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Dic MicroMoleBiology PDF
Dic MicroMoleBiology PDF
Dic MicroMoleBiology PDF
Preface
This edition follows the style of previous editions. It has similar aims, and was written with the same
enthusiasm and care.
It is vital that readers be aware of the type of alphabetization used in the Dictionary. A glance at Notes
for the User particularly the first paragraph is essential.
September 2001
vii
we are grateful to Michael Dixon, Patricia Sharp, and Prue Theaker at John Wiley & Sons, Chichester, for
their enthusiastic and efficient cooperation in the production of the book.
Paul Singleton & Diana Sainsbury
Clyst St Mary, Devon, April 1987
viii
atoxyl
ATP
ATP synthase
ATPase
RecA protein
recapitulation theory
recB gene
RecBC pathway
When a hyphen connects two complete words, or occurs between a letter (or group of letters) and a word,
the hyphen is regarded as a space; however, if a hyphen is used to link a prefix to a word (i.e., if the letters
preceding the hyphen form a part-word which cannot stand alone) the term is alphabetized as though it were
a single, non-hyphenated word. (In a few cases an entry heading contains words which can be written as
separate, hyphenated or non-hyphenated words, or closed up as a single word: e.g. red water fever, red-water
fever, redwater fever; in such cases an entry or cross-reference has been included in both possible positions.)
Examples:
BL-type starter
bla gene
black beans
Black beetle virus
M
M antigen
M-associated protein
M bands
nonsense mutation
nonsense suppressor
non-specific immunity
non-specific immunization
preaxostyle
pre-B cell
prebuccal area
precipitation
When a Greek letter forms a significant part of an entry heading it is counted as a word and is alphabetized
as spelt (i.e., a as alpha, b as beta, etc: see Appendix VI for the Greek alphabet). A Greek letter is ignored
for the purposes of alphabetization if it is a relatively minor qualification: e.g., part of a chemical designation
(which can usually be replaced by a number, as in b-hydroxybutyrate, = 3-hydroxybutyrate). Examples:
Delhi boil
1
delta agent
d antigen
MTOC
Mu
mu chain
pHisoHex
fX phage group
Phlebia
Phlebotomus
polyhedrosis
poly-b-hydroxyalkanoate
poly-b-hydroxybutyrate
Polyhymenophorea
A number which forms part of an entry heading affects the position of that entry only if the number
immediately follows a letter or word (but cf. chemical names, below). A number which precedes a letter
or word is usually ignored, although in the few cases where a number is the first and main part of an
entry heading it is alphabetized as spelt. Letternumber combinations come after a letterspace but before
letterletter combinations, as in the illustrative sequence A, A2, A2A, A3, A22, AA, ABA etc. Roman
numerals are treated as ordinary numbers (I as 1, II as 2 etc). (The reader should bear in mind that, in an
unfamiliar term, I could be a letter I or a Roman one, and its location in the Dictionary will be affected
accordingly; similarly, V could be letter V or Roman five. O and 0 (zero) may also be confused. If in
doubt check both possible positions.) Examples:
bacteriophage
bacteriophage
bacteriophage
bacteriophage
Pf2
fI
fII
f6
D loop
D period
12D process
D-type particles
Fitz-HughCurtis syndrome
fivefivefive test
five-kingdom classification
fivethreetwo symmetry
ix
T1 side-chains
T-2 toxin
T2H test
T7 phage group
Subscript/superscript numbers and letters are alphabetized as though they were ordinary numbers and letters
(except in the case of ion designations: see below). Examples:
avoparcin
aw
axenic
axial fibrils
B virus
B12 coenzymes
B663
BabesErnst granules
C3 convertase
C3 cycle
C3bina
C5 convertase
CO2
CO2 -stat
CoA
coactin
Primes, apostrophes and other non-alphabetizable symbols (including e.g. plus, minus and % signs) are
ignored. Examples:
brown rust
Brownes tubes
Brownian movement
Browns tubes
F antigens
F+ donor
F-duction
F factor
Gautieriales
Gazdar murine sarcoma virus
GC%
GC type
In chemical names qualifications such as D-, L-, N -, o-, p-, numbers and Greek letters, as well as hyphens
between parts of chemical names, are all ignored for the purposes of alphabetization. Examples:
acetyl-CoA synthetase
N-acetyl-D-glucosamine
acetylmethylcarbinol
N-acetylmuramic acid
diazomycin A
6-diazo-5-oxo-L-norleucine
diazotroph
dibromoaplysiatoxin
methylmethane sulphonate
N-methyl-N -nitro-N-nitrosoguanidine
N-methyl-N-nitrosourea
Methylobacterium
In entry headings which include an ion designation, the ion is treated as a word, the charge being ignored;
thus, H+ is regarded as H, Ca2+ as Ca, etc. Examples:
H antigens
H+ -ATPase
H+ /2e ratio
H-lysin
H+ /P ratio
H+ -PPase
H strand
H-1 virus
K cells
K+ pump
K+ transport
K virus
Na+ -ATPase
Na+ -motive force
Na+ pump
nabam
2. Cross-references. References from one entry to another within the Dictionary are indicated by SMALL
CAPITAL letters. In order to effect maximum economy of space, information given in any particular entry is
seldom repeated elsewhere, and cross-referencing has been extensively employed to ensure continuity of
information. In some cases a complete understanding of an entry, or an appreciation of context, is dependent
on a knowledge of information given in other entries; where it is particularly important to follow up a crossreference, the cross-reference is followed by q.v.. In other cases a cross-reference may be used to link one
topic with another of related interest, or to extend the scope of a given topic in one or more directions; in
such cases a cross-reference is usually preceded by see also or cf.. (N.B. For a variety of reasons, not
every microbiological term or taxon used in the text is cross-referred even though most of these terms
and taxa are defined in the Dictionary; the reader is therefore urged to use the Dictionary for any unfamiliar
term or taxon.)
When reading an entry for a genus, family or other taxon, it is especially important to follow up, when
indicated, a cross-reference to the higher taxon to which it belongs. An entry for a given higher taxon gives
the essential features applicable to all members of that taxon, and such features are usually not repeated in
the entries for each of the constituent lower-ranked taxa; thus, in failing to follow up such cross-references,
the reader will forfeit fundamental information relating to the lower taxon in question.
In some cases an entry heading is followed simply by See CROSS-REFERENCE. This is not intended to
indicate that the two terms are synonymous (usually they are not); such referral signifies only that the
meaning of the term is given under the heading indicated. When the entry heading and cross-reference are
synonymous, this is indicated by Syn., thus: entry heading Syn. CROSS-REFERENCE.
3. External references. References to papers, articles etc in books or journals are given in square brackets.
In order to save space, books are referred to by a Book ref. number, and journal titles are abbreviated
x
somewhat more than is usual; keys to book reference numbers and journal title abbreviations can be found
at the end of the Dictionary (after the Appendices).
A book reference is usually quoted as a source of general background information for the reader, while
papers in journals are usually quoted for specific details of current information (or for reviews) and/or for
their references to other literature in the field. We should emphasize that the papers we have cited are not
necessarily (and are commonly not) those which were the first to report a particular fact, finding or theory;
rather, we have chosen, where possible, to cite the most recent references available to us, so that the reader
is referred to current information and can, if he wishes, trace the earlier literature via references given in
the cited papers. We should also point out that the quoting of a single reference in an entry is not intended
to indicate that the entry was written solely from information in that paper or book. In relatively few cases
does the information in an entry derive from a single source; in the great majority of entries the information
has been derived from, or checked against, a range of sources, but limitations of space have necessarily
prevented us from citing all of them.
4. Numbered definitions. In some cases a term is used with different meanings by different authors, or it
may have different meanings in different contexts; for such a term the various definitions are indicated by
(1), (2), (3), etc. The order in which the numbered definitions occur is not intended to reflect in any way
appropriateness or frequency of usage.
5. Taxonomy. See entries ALGAE, BACTERIA, FUNGI, PROTOZOA and VIRUS for some general comments on the
taxonomy of each of these groups of microorganisms. Each of these entries (except that on bacteria) provides
a starting point from which the reader can, via cross-references, follow through a hierarchical system down
to the level of genus and, in many cases, species and below; similarly, the hierarchy can be ascended from
genus upwards.
6. The Greek alphabet. See Appendix VI.
xi
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
A
A
(Angstr
A
om unit) 1010 m (= 101 nm).
25A See INTERFERONS.
A-DNA See DNA.
a-factor See MATING TYPE.
A layer An S LAYER associated with virulence in strains of
Aeromonas salmonicida.
A-protein In TOBACCO MOSAIC VIRUS: a mixture of small
oligomers and monomers of coat protein subunits which occur in
equilibrium with the larger disc aggregates under conditions of
physiological pH and ionic strength; coat protein occurs mainly
as A-protein under conditions of high pH and low ionic strength.
(cf. PROTEIN A.)
A site (of a ribosome) See PROTEIN SYNTHESIS.
A-tubule (A-subfibre) See FLAGELLUM (b).
A-type inclusion body See POXVIRIDAE.
A-type particles Intracellular, non-infectious, retrovirus-like particles. Many embryonic and transformed mouse cells contain
retrovirus-like intracisternal A-type particles (IAPs) which
form by budding at the endoplasmic reticulum; these particles have reverse transcriptase activity and an RNA genome
coding for the structural protein of the particles. The mouse
genome contains ca. 1000 copies (per haploid genome) of
DNA sequences homologous to IAP-associated RNA; these
sequences appear to be capable of transposition within the
mouse genome probably via an RNA intermediate [Book
ref. 113, pp. 273279], i.e., they may be RETROTRANSPOSONS.
Some A-type particles are non-enveloped precursors of B-type
particles (see TYPE B ONCOVIRUS GROUP).
A23187 An IONOPHORE which transports divalent cations, particularly Ca2+ ; it can effect the transmembrane exchange of 1Ca2+
(or 1Mg2+ ) for 2H+ without causing perturbation in the gradients of other monovalent cations.
AAA ATPases ATPases associated with diverse cellular activities. AAA ATPases occur e.g. in PEROXISOMES and as components of eukaryotic PROTEASOMES.
AAA pathway AMINOADIPIC ACID PATHWAY.
AAC Aminoglycoside acetyltransferase (see AMINOGLYCOSIDE
ANTIBIOTICS).
AAD Aminoglycoside adenylyltransferase (see AMINOGLYCOSIDE
ANTIBIOTICS).
AAS Aminoalkylsilane (3-aminopropyltriethoxy-silane, APES;
3(triethoxysilyl)-propylamine, TESPA): a reagent used for binding a tissue section to the surface of a glass slide (e.g. for in situ
hybridization); it reacts with silica glass and provides aminoalkyl
groups which bind to aldehyde or ketone groups in the tissue
section.
aat gene In Escherichia coli: a gene whose product promotes
the early degradation of those proteins whose N-terminal amino
acid is either arginine or lysine. aat encodes an amino acid
transferase which catalyses the addition of a leucine or phenylalanine residue to the N-terminus of the protein; this destabilizes
the protein, facilitating its degradation. (See also N-END RULE.)
AatII See RESTRICTION ENDONUCLEASE (table).
Aaterra See ETRIDIAZOLE.
AAUAAA locus See MRNA (b).
AAV Adeno-associated virus: see DEPENDOVIRUS.
ab (immunol.) ANTIBODY.
ABC protein
ABC adheres non-specifically to biotin). Peroxidase (and hence
antigen) is detected by incubating the section with e.g. H2 O2
and diaminobenzidine (which results in the antigenic site being
stained brown) or H2 O2 and 4-chloro-1-naphthol (resulting in a
blue stain).
The ABC method can be used for paraffin-embedded sections,
frozen sections, and smears. Endogenous (tissue or cell) peroxidase may be quenched e.g. with H2 O2 in methanol.
ABC protein See ABC TRANSPORTER.
ABC transporter (traffic ATPase) A type of TRANSPORT SYSTEM
which, in bacteria, consists typically of a multiprotein complex
in the cell envelope, two of the proteins having a specific ATPbinding site (termed the ATP-binding cassette; ABC) on their
cytoplasmic surface; a (bacterial) protein with an ABC site
has been called an ABC protein or an ABC subunit. In
eukaryotes, an ABC transporter generally consists of a single
polypeptide chain which also has two ATP-binding sites.
Transport mediated by an ABC transporter is energized by ATP
hydrolysis at the ABC sites. [ATP-hydrolysing regions of ABC
transporters: FEMS Reviews (1998) 22 120.] (See also PROTEIN
SECRETION.)
A given type of ABC transporter imports or exports/secretes
certain type(s) of ion or molecule. Collectively, these transporters import or secrete a wide range of substances, including
ions, sugars and proteins; for example, some import nutrients,
or ions for OSMOREGULATION, while others secrete antibiotics
or protein toxins. The LmrA transporter in Lactococcus lactis
mediates an efflux system that extrudes amphiphilic compounds
and appears to be functionally identical to the mammalian Pglycoprotein that mediates multidrug-resistance [Nature (1998)
391 291295]. The AtrB transporter of Aspergillus nidulans
mediates energy-dependent efflux of a range of fungicides [Microbiology (2000) 146 19871997].
ABC transporters occur e.g. in Gram-positive and Gramnegative bacteria, members of the Archaea, and in higher
animals, including man. In man, certain inheritable diseases (e.g.
CYSTIC FIBROSIS and adrenoleukodystrophy) result from defective
ABC transporters.
The bacterial ABC importer is commonly called a BINDING
PROTEIN-DEPENDENT TRANSPORT SYSTEM (q.v.). (See also ABC
EXPORTER.)
ABE process An industrial process in which acetone, butanol
and ethanol are produced by the fermentation of e.g. molasses
by Clostridium acetobutylicum. (See also ACETONEBUTANOL
FERMENTATION.)
Abelson murine leukaemia virus (Ab-MuLV) A replicationdefective, v-onc+ MURINE LEUKAEMIA VIRUS isolated from a
prednisolone-treated BALB/c mouse inoculated with Moloney
murine leukaemia virus (Mo-MuLV). Ab-MuLV apparently
arose by recombination between Mo-MuLV and mouse
c-abl sequences; the v-abl product has tyrosine kinase activity.
(See also ABL.) Ab-MuLV induces B-cell lymphoid leukaemia
with a short latent period (34 weeks). [Abelson viruscell
interactions: Adv. Imm. (1985) 37 7398.]
abequose (3,6-dideoxy-D-galactose) A sugar, first isolated from
Salmonella abortusequi, which occurs in the O-specific chains
of the LIPOPOLYSACCHARIDE in certain Salmonella serotypes and
which contributes to the specificity of O antigen 4 in group B
salmonellae (see KAUFFMANNWHITE CLASSIFICATION).
aberration (chromosomal) See CHROMOSOME ABERRATION.
abhymenial Of or pertaining to a region opposite or away from
the HYMENIUM.
abiogenesis (spontaneous generation) The spontaneous formation of living organisms from non-living material; apart from
Acetobacter
Acantharea A class of marine, mostly planktonic protozoa
(superclass ACTINOPODA) which have elaborate skeletons composed of strontium sulphate; typically, the skeleton consists of
10 spines arranged diametrically in the (more or less spherical)
cell, or 20 spines which radiate from the cell centre (where they
may or may not be joined at their bases, according to species).
In many species the cell contains a central capsule (cf. RADIOLARIA); many species contain zooxanthellae. Five orders are
recognized; genera include e.g. Acanthochiasma, Acanthometra,
Astrolophus, Gigartacon.
Acanthochiasma See ACANTHAREA.
Acanthocystis See CENTROHELIDA.
Acanthoeca See CHOANOFLAGELLIDA.
Acanthometra See ACANTHAREA.
acanthopodia See ACANTHAMOEBA.
acaricide Any chemical which kills mites and ticks (order
Acarina).
Acarospora A genus of LICHENS (order LECANORALES). Thallus:
crustose, areolate, with prominent areolae. Apothecia are embedded in the areolae; ascospores: very small, many per ascus.
All species are saxicolous, some are ENDOLITHIC; A. smaragdula
occurs on rocks and slag rich in heavy metals.
Acarpomyxea A class of protozoa (superclass RHIZOPODA) with
characteristics intermediate between those of the naked amoebae and the plasmodial slime moulds: they form small plasmodia
(or large uninucleate plasmodium-like forms) which are usually
branched and which sometimes anastomose to form a coarse
reticulum. Spores, fruiting bodies and tests are absent; cysts are
produced by some species. Orders: Leptomyxida (soil and freshwater organisms, e.g. Leptomyxa [Book ref. 133, pp. 143144],
Rhizamoeba) and Stereomyxida (marine organisms, e.g., Corallomyxa, Stereomyxa).
Acaryophrya See GYMNOSTOMATIA.
Acaulopage See e.g. NEMATOPHAGOUS FUNGI.
Acaulospora See ENDOGONALES.
acceptor site (of a ribosome) See PROTEIN SYNTHESIS.
acceptor splice site See SPLIT GENE (a).
accessory cells (immunol.) Those cells which, together with B
LYMPHOCYTES and/or T LYMPHOCYTES, are involved in the expression of humoral and/or cell-mediated immune responses; they
include e.g. MACROPHAGES, DENDRITIC CELLS, and LANGERHANS
CELLS.
accessory pigments In PHOTOSYNTHESIS: those pigments contained in LIGHT-HARVESTING COMPLEXES.
AcCoA Acetyl-COENZYME A.
Ace toxin (Vibrio cholerae) See BACTERIOPHAGE CTX8.
acellular (non-cellular) (1) Refers to an organism, usually a
protozoon, which consists essentially of a single cell but in
which occur functionally specialized regions sometimes regarded
as analogous to the organs and tissues of a differentiated
multicellular organism. (2) Refers to an organism (e.g. a VIRUS)
or structure (e.g. the stalk of ACYTOSTELIUM) which is not
CELLULAR in any sense. (3) Not divided into cells (as e.g. in
a PLASMODIUM).
acellular slime moulds See MYXOMYCETES.
acentric (of a chromosome) Having no CENTROMERE.
acephaline gregarines See GREGARINASINA.
acer tar spot See RHYTISMA.
acervulus A flat or saucer-shaped fungal STROMA supporting
a mass of typically short and densely-packed conidiophores;
acervuli commonly develop subcuticularly or subepidermally in
a plant host, becoming erumpent at maturity, i.e., rupturing the
overlying plant tissue to allow dispersal of the conidia. Some
acervuli bear setae (see SETA).
Acetobacteraceae
Cells: typically ovoid or rod-shaped, 0.60.8 1.04.0 m,
non-motile or with peritrichous or lateral flagella. Most strains
are catalase-positive. Typically, ethanol is oxidized to acetic
acid, and acetic acid is oxidized (overoxidation) to CO2 (cf.
GLUCONOBACTER). Principal substrates include e.g. ethanol, glycerol and lactate; most strains grow well on glucoseyeast
extractCaCO3 agar (GYC agar), forming round pale colonies.
(See also CARR MEDIUM.) Some strains form CELLULOSE (see
PELLICLE (1)). Sugars appear to be metabolized primarily via
the HEXOSE MONOPHOSPHATE PATHWAY and the TCA CYCLE; phosphofructokinase seems to be absent (cf. Appendix I(a)). The
ENTNERDOUDOROFF PATHWAY appears to occur only in cellulosesynthesizing strains. Growth on HOYERS MEDIUM appears to
involve enzymes of the glyoxylate shunt. Optimum growth temperature: 2530 C. GC%: ca. 5165. Type species: A. aceti.
A. aceti. Ketogenic with glycerol or sorbitol substrates;
5-ketogluconic acid (but not 2,5-diketogluconic acid) formed
from D-glucose. No diffusible brown pigments are formed on
GYC agar. Grows on sodium acetate.
A. hansenii. Ketogenic with glycerol or sorbitol substrates; 5ketogluconic acid (but not 2,5-diketogluconic acid) is formed
by some strains from D-glucose. No growth on sodium acetate.
No diffusible brown pigments are formed on GYC agar. (cf.
A. xylinum.)
A. liquefaciens. Brown diffusible pigments are formed on
GYC agar. 2,5-Diketogluconic acid is formed from D-glucose.
Ketogenic with glycerol as substrate.
A. pasteurianus. Ketogluconic acids are not formed from Dglucose. No brown diffusible pigments are formed on GYC
agar. Some strains (formerly called A. peroxydans) are catalasenegative. (cf. A. xylinum.)
A. peroxydans. See A. pasteurianus.
A. suboxydans. See GLUCONOBACTER.
A. xylinum. Cellulose-producing strains formerly classified as
a subspecies of A. aceti, then distributed between the two species
A. hansenii and A. pasteurianus; A. xylinum has now been
accepted as a revived name for cellulose-forming and celluloseless, acetate-oxidizing strains [IJSB (1984) 34 270271].
[Book ref. 22, pp. 268274.]
Acetobacteraceae A family of aerobic, oxidase-negative, chemoorganotrophic, Gram type-negative bacteria which typically oxidize ethanol to acetic acid. Metabolism: strictly respiratory
(oxidative), with O2 as terminal electron acceptor. Growth
occurs optimally at ca. pH 56. The organisms occur e.g. in
acidic, ethanol-containing habitats. GC%: ca. 5165. Two genera: ACETOBACTER (type genus), GLUCONOBACTER [Book ref. 22,
pp. 267278].
Acetobacterium A genus of Gram-negative, obligately anaerobic
bacteria which occur in marine and freshwater sediments [IJSB
(1977) 27 355361]. Cells: polarly flagellated ovoid rods,
ca. 1.0 2.0 m, often in pairs. The type species, A. woodii,
can carry out a homoacetate fermentation of e.g. fructose,
glucose or lactate, or can grow chemolithoautotrophically (see
ACETOGENESIS); it contains group B PEPTIDOGLYCAN. Optimum
growth temperature: 30 C. GC%: ca. 39. (See also ANAEROBIC
DIGESTION.)
acetogen (1) Any bacterium (e.g. Acetobacterium woodii,
Clostridium aceticum, C. thermoaceticum) which produces
acetate as the main product from certain sugars (via
homoacetate fermentation and reduction of carbon dioxide)
and (in some strains) from carbon dioxide and hydrogen (see
ACETOGENESIS).
(2) (hydrogenogen; proton-reducing acetogen) Any bacterium which can use protons as electron acceptors for the
Acinetobacter
A-CGT See IMMUNOSORBENT ELECTRON MICROSCOPY.
achlorophyllous Syn. ACHLOROTIC.
achlorotic (achlorophyllous) Lacking chlorophyll. (cf. APOCHLOROTIC.)
Achlya
A genus of aquatic fungi (order SAPROLEGNIALES) in
which the thallus is characteristically a branched, coenocytic
mycelium; the width of the hyphae varies with species. Although
Achlya species are typically saprotrophic some have been
reported to parasitize rice plants. (See also DIPLANETISM, HETEROTHALLISM and PHEROMONE.)
Achnanthes See DIATOMS.
Acholeplasma
A genus of facultatively anaerobic, ureasenegative bacteria (family ACHOLEPLASMATACEAE) which are associated with various vertebrates (and possibly with invertebrates
and plants), and which also occur e.g. in soil and sewage and as
contaminants in TISSUE CULTURES. Cells: non-motile cocci (minimum diam. ca. 300 nm) or filaments (typically ca. 25 m
in length); carotenoid pigments occur in some species. The
organisms resemble Mycoplasma spp in their general properties, but differ e.g. in that their growth is sterol-independent,
and in that NADH oxidase occurs in the cytoplasmic membrane
rather than in the cytoplasm. Acholeplasma spp are susceptible to various ACHOLEPLASMAVIRUSES. GC%: ca. 2636. Type
species: A. laidlawii; other species: A. axanthum, A. equifetale,
A. granularum, A. hippikon, A. modicum, A. morum, A. oculi.
[Book ref. 22, pp. 775781.]
Acholeplasmataceae A family of bacteria of the order MYCOPLASMATALES; species of the sole genus, ACHOLEPLASMA, differ
from the other members of the order e.g. in that their growth
is not sterol-dependent. [Proposal for re-classifying Acholeplasmataceae as the order Acholeplasmatales: IJSB (1984) 34
346349.]
acholeplasmaviruses BACTERIOPHAGES which infect Acholeplasma species: see PLECTROVIRUS, PLASMAVIRIDAE, MV-L3 PHAGE
GROUP.
achromat (achromatic objective) An objective lens (see MICROSCOPY) in which chromatic aberration has been corrected for
two colours (usually red and blue), and spherical aberration
has been corrected for one colour (usually yellowgreen). (cf.
APOCHROMAT.) A FLAT-FIELD OBJECTIVE LENS of this type is called
a planachromat.
Achromobacter An obsolete bacterial genus.
achromogenic Refers to an organism (or e.g. reagent) which does
not produce pigment (or colour); used e.g. of non-pigmented
strains of normally CHROMOGENIC organisms.
achromycin See TETRACYCLINES.
aciclovir A spelling used by some authors for the drug ACYCLOVIR.
acicular Needle-shaped.
Aciculoconidium A genus of fungi (class HYPHOMYCETES) which
form budding ovoid or ellipsoidal cells (occurring singly or in
short chains or clusters) as well as branched septate hyphae.
Conidia are formed terminally and are acicular, rounded at
one end and pointed at the other. NO3 is not assimilated.
One species: A. aculeatum (formerly Trichosporon aculeatum),
isolated from Drosophila spp. [Book ref. 100, pp. 558561.]
acid dye See DYE.
acid-fast organisms Organisms (e.g. Mycobacterium spp) which,
once stained with an ACID-FAST STAIN, cannot be decolorized by
mineral acids or by mixtures of acid and ethanol.
acid-fast stain Any stain used to detect or demonstrate ACID-FAST
ORGANISMS e.g. ZIEHLNEELSENS STAIN, AURAMINERHODAMINE
STAIN.
AcLVs
as a chemoattractant for cell aggregation. Acrasins are a diverse
group of substances; they include cAMP in Dictyostelium discoideum (q.v.), a pterin in Dictyostelium lacteum [PNAS (1982)
79 62706274], and a dipeptide, glorin, in Polysphondylium
violaceum (q.v.).
Acrasiomycetes (acrasid cellular slime moulds; acrasids) A class
of cellular SLIME MOULDS (division MYXOMYCOTA) in which the
vegetative phase consists of amoeboid cells that form lobose
pseudopodia; the amoebae aggregate (without streaming) to form
a pseudoplasmodium which is not slug-like and does not migrate
(cf. DICTYOSTELIOMYCETES). The pseudoplasmodium gives rise to
multispored fruiting bodies which may have long or short stalks
(but no cellulosic stalk tube) bearing e.g. simple globular sori or
branched or unbranched chains of spores. Flagellated cells have
been observed in only one species (Pocheina rosea). Sexual
processes are unknown. Acrasids occur in various habitats: e.g.
dung, tree-bark, dead plant materials, etc. Genera include Acrasis,
Copromyxa, Copromyxella, Fonticula, Guttulinopsis, Pocheina
(formerly Guttulina).
(Zoological taxonomic equivalents of the Acrasiomycetes
include the class Acrasea of the MYCETOZOA, and the class
Acrasea of the RHIZOPODA.)
Acrasis See ACRASIOMYCETES.
Acremonium
A genus of fungi of the class HYPHOMYCETES;
teleomorphs occur in e.g. Emericellopsis and Nectria. The genus
includes organisms formerly classified as species of Cephalosporium [for references see MS (1986) 3 169170]. Acremonium spp form septate mycelium; conidia, often in gelatinous
masses, are produced from phialides which develop from simple, single branches of the vegetative hyphae. A. kiliense (=
Cephalosporium acremonium) produces cephalosporin C (see
CEPHALOSPORINS). (See also MADUROMYCOSIS.)
acridine orange (basic orange, or euchrysine; 3,6-bis(dimethylamino)-acridinium chloride) A basic dye and FLUOROCHROME
used e.g. in fluorescence MICROSCOPY to distinguish between
dsDNA (which fluoresces green) and ss nucleic acids (which
fluoresce orange-red). Sublethal concentrations of the dye are
used for CURING plasmids. (See also ACRIDINES.)
acridines Heterocyclic compounds which include acridine and
its derivatives. At low concentrations, aminoacridines (e.g.
proflavine (3,6-diaminoacridine), QUINACRINE) appear to bind to
dsDNA (or to double-stranded regions of ssDNA) primarily as
INTERCALATING AGENTS. At higher concentrations there is also a
weaker, secondary type of binding in which the acridine binds
to the outside of dsDNA or to ssDNA or ssRNA; the two types
of binding may account for the differential staining of DNA
and RNA by ACRIDINE ORANGE. [Book ref. 14, pp. 274306.]
Acridines inhibit DNA and RNA synthesis and cause e.g.
FRAMESHIFT MUTATIONS. They are used e.g. as antimicrobial
agents (see e.g. ACRIFLAVINE), as mutagens, and as fluorescent
stains for nucleic acids; they also have potential antitumour
activity. (See also CURING (2).)
As antimicrobial agents, acridines are active against a wide
range of bacteria, but they are not sporicidal; some are active
against certain parasitic protozoa (see e.g. QUINACRINE and
KINETOPLAST) and inhibit the replication of certain viruses.
Activity is not significantly affected by proteinaceous matter.
[Acridines as antibacterials (review): JAC (2001) 47 113.]
As mutagens, acridines may be effective in replicating bacteriophages but are generally not effective in bacteria. However,
compounds in which an acridine nucleus is linked to an alkylating side-chain ICR compounds (ICR = Institute for Cancer Research) can induce frameshift and other mutations in
bacteria.
Most strains can grow on a mineral salts medium containing an organic carbon source such as acetate, ethanol or lactate as the sole source of carbon and energy; some can use
amino acids (e.g. L-leucine, ornithine) and/or pentoses (e.g. Larabinose, D-xylose), and some are able to degrade e.g. benzoate,
n-hexadecane and alicyclic compounds (see HYDROCARBONS).
Acinetobacters appear to contain all the enzymes of the TCA
CYCLE and the glyoxylate cycle. Many carbohydrates can be
used. Most strains in the A. calcoaceticusA. baumannii complex (and in certain other groups) can form acid from glucose
(oxidatively), but many (e.g. most strains designated A. lwoffii )
cannot. The optimal growth temperature is typically 3335 C.
GC%: 3847. Type species: A. calcoaceticus.
The taxonomy of Acinetobacter is confused and unsatisfactory. Emended descriptions of the two species A. calcoaceticus
and A. lwoffii, and proposals for four new species (A. baumannii,
A. haemolyticus, A. johnsonii and A. junii ), were published in
1986 [IJSB (1986) 36 228240]. Since then, a number of
adjustments have been made to the taxonomic structure of the
genus. [Taxonomy, and epidemiology of Acinetobacter infections: RMM (1995) 6 186195.]
Acinetobacters have been isolated in a number of hospitalassociated (and other) outbreaks of disease, often as part
of a mixed infection; in most cases such infections involve
glucolytic strains of the A. calcoaceticusA. baumannii complex particularly A. baumannii (also called group 2, or
genospecies 2). The most common manifestations of disease
include septicaemia and infections of the urinary tract, lower
respiratory tract and central nervous system. Transmission may
occur by direct contact or may involve the airborne route. Acinetobacters have been reported to survive on dry surfaces for at
least as long as e.g. Staphylococcus aureus.
One problem associated with the pathogenic role of Acinetobacter is that these organisms appear easily to acquire resistance
to antibiotics so that they have the potential to develop as
multiresistant pathogens; currently, for example, acinetobacters
are reported to be resistant to most b-lactam antibiotics, particularly penicillins and cephalosporins, and to chloramphenicol
and trimethoprimsulphamethoxazole. [Mechanisms of antimicrobial resistance in A. baumannii: RMM (1998) 9 8797.]
AcLVs AVIAN ACUTE LEUKAEMIA VIRUSES.
acne A chronic skin disorder characterized by increased sebum
production and the formation of comedones (blackheads and
whiteheads) which plug the hair follicles. Propionibacterium
acnes, present in the pilosebaceous canal (see SKIN MICROFLORA),
may play a causal role; it produces a lipase that hydrolyses
sebum triglycerides to free fatty acids, and these can cause
inflammation and comedones [JPed (1983) 103 849854].
Treatment: e.g. topical SALICYLIC ACID or benzoyl peroxide; the
latter has keratinolytic activity and exerts bactericidal action on
P. acnes by releasing free-radical oxygen.
Aconchulinida See FILOSEA.
aconitase See Appendix II(a) and NITRIC OXIDE.
Aconta Algae of the RHODOPHYTA. (cf. CONTOPHORA.)
acquired immune deficiency syndrome See AIDS.
acquired immunity (1) SPECIFIC IMMUNITY acquired through
exposure to a given antigen. (2) PASSIVE IMMUNITY. (3) NONSPECIFIC IMMUNITY acquired through exposure to certain viruses
(see e.g. INTERFERONS) or by immunization with BCG.
Acrasea See ACRASIOMYCETES.
acrasids See ACRASIOMYCETES.
acrasin In cellular slime moulds: a generic term for a chemotactic substance which is produced by cells and which serves
6
actinoidin
(6)
(5)
(4)
(7) 7
(8) 6
(3)
(2)
N
5
10
(9)
(10)
(1)
acriflavine (acriflavin; syn. euflavin) 3,6-Diamino-10-methylacridinium chloride or (according to some authors) a mixture of this
compound and 3,6-diaminoacridine (proflavine). Acriflavine is
soluble in water and in ethanol, and has been used as an ANTISEPTIC.
(See also ACRIDINES.)
acro- Prefix meaning tip or outermost part.
Acrocordia See PYRENULALES.
acrolein (CH2 =CHCHO) An aldehyde used e.g. for preFIXATION; it penetrates tissues more rapidly than GLUTARALDEHYDE.
acronematic Refers to a eukaryotic FLAGELLUM which is smooth
and tapers to a fine point.
acropetal development Development from the base, or point
of attachment, towards the tip; e.g., in a chain of acropetally
developing spores the first-formed spores occupy positions in
the chain nearest the base of the spore-bearing structure, while
spores formed later occupy positions in the distal parts of the
chain. (cf. BASIPETAL DEVELOPMENT.)
acropleurogenous Located both at the tip and on the sides of an
elongated structure.
Acrosiphonia A genus of branched, filamentous, siphonocladous
green algae (division CHLOROPHYTA).
Acrospermum See CLAVICIPITALES.
acrylate pathway See PROPIONIC ACID FERMENTATION.
ActA protein (Listeria monocytogenes) See LISTERIOSIS.
actaplanin See VANCOMYCIN.
Actidione Syn. CYCLOHEXIMIDE.
actin (1) A protein, found in most types of eukaryotic cell, which
can polymerize (reversibly) to form non-contractile filaments
(microfilaments) that are involved e.g. in maintaining cell
shape and structure (see e.g. CYTOSKELETON) and (together
with MYOSIN) in CAPPING (sense 3), amoeboid movement (see
PSEUDOPODIUM), CYTOPLASMIC STREAMING, PHAGOCYTOSIS, and (in
higher animals) muscle contraction.
Actins from various sources are similar in structure. The
monomeric form (G-actin) is a globular protein (MWt ca.
42000) consisting of ca. 375 amino acid residues; each molecule
can bind one molecule of ATP. In most non-muscle cells,
G-actin occurs in dynamic equilibrium with the polymerized
(filamentous) form, F-actin, which consists of a helical, doublestranded chain of monomers ca. 7 nm thick. Although F-actin
is itself non-contractile, its interaction with myosin can cause
microfilaments to slide relative to one another thereby bringing
about movements and contractions in structures bound to the
microfilaments. During the polymerization of G-actin ATP is
hydrolysed; as in the assembly of MICROTUBULES, energy is
not essential for but increases the rate of polymerization.
Polymerization and depolymerization can occur at both ends of
a microfilament, but one of the ends may grow (or depolymerize)
at a greater rate than the other. (See also CAPPING sense 2.)
7
Actinomadura
Actinomadura
A genus of bacteria (order ACTINOMYCETALES,
wall type III; group: maduromycetes) which occur e.g. in soil;
some species (A. madurae, A. pelletieri ) can be pathogenic in
man (see MADUROMYCOSIS). The organisms form a branching,
usually stable, substrate mycelium, but (spore-forming) aerial
mycelium may be common or rare according to species; some
species contain only trace amounts of madurose, or none
at all. GC%: reported to be within the range 6578. Type
species: A. madurae. [Taxonomic studies on Actinomadura and
Nocardiopsis: JGM (1983) 129 34333446; ecology, isolation
and cultivation: Book ref. 46, pp. 21032117.]
Actinomucor See MUCORALES.
Actinomyces A genus of asporogenous bacteria (order ACTINOMYCETALES; wall type varies with species); species occur in
warm-blooded animals e.g. as part of the microflora of the
mucous membranes (particularly in the mouth) and can act as
opportunist pathogens. The organisms occur as rods, branched
rods or filaments, or as a rudimentary mycelium. All species
can grow anaerobically, or under reduced partial pressure of
oxygen; growth in vitro occurs readily on rich media at 37 C,
and is typically enhanced if the partial pressure of carbon
dioxide is increased. Carbohydrates are fermented anaerogenically acetic, lactic and succinic acids being the main acidic end
products of glucose fermentation in PYG MEDIUM. Most species
are catalase-negative; A. viscosus is catalase-positive. GC%: ca.
5773. Type species: A. bovis.
A. bovis (wall type VI) and A. israelii (wall type V) can
cause chronic disease in animals and man (see ACTINOMYCOSIS); A. naeslundii and A. viscosus (both wall type V) can
cause periodontitis e.g. in rodents. (See also COAGGREGATION.)
A. pyogenes (formerly Corynebacterium pyogenes [JGM (1982)
128 901903]) is the cause of summer mastitis in cattle, and
is often isolated from pyogenic lesions in cattle, pigs and other
animals; A. pyogenes typically occurs as short rods or coryneforms which secrete a soluble haemolysin. A. hordeovulneris
[IJSB (1984) 34 439443] is a causal agent of actinomycosis
in dogs.
Actinomycetales An order of GRAM TYPE-positive, typically aerobic bacteria; species range from those which occur as cocci
and/or rods to those which form a well-developed, branching SUBSTRATE MYCELIUM and/or AERIAL MYCELIUM, and which
may form sophisticated structures such as sclerotia, sporangia and synnemata. (cf. ACTINOMYCETE.) Most members of
the order have a GC%>55, thus distinguishing them from
species of the other major subbranch of Gram-positive bacteria: the ClostridiumBacillusThermoactinomyces line (but cf.
CORYNEBACTERIUM, RENIBACTERIUM and THERMOACTINOMYCES).
Phylogenetic relationships between actinomycetes are indicated
by 16S rRNA oligonucleotide cataloguing and nucleic acid
hybridization; within the order, groups of genera can be distinguished on the basis of e.g. the chemical nature of the cell
wall and the lipid profiles of the organisms. [The system of
classification adopted in the Dictionary is based on the scheme
proposed in Book ref. 73, pp. 7164.]
Actinomycetes are widespread in nature, occurring typically in soil, composts (see COMPOSTING) and aquatic habitats;
most species are free-living and saprotrophic, but some form
symbiotic associations (see e.g. ACTINORRHIZA) and others are
pathogenic in man, other animals, and plants (see e.g. ACTINOMYCOSIS, DERMATOPHILOSIS, JOHNES DISEASE, POTATO SCAB, and
TUBERCULOSIS). The organisms are chemoorganotrophs; collectively they can degrade a wide range of substances which include
e.g. agar, cellulose, chitin, keratin, paraffins and rubber. Some
species produce important antibiotics (see e.g. STREPTOMYCES).
Actinosphaerium
are involved in antibiotic production. Genetic analyses have been
carried out by methods involving e.g. conjugation and protoplast
fusion.
Genera include: ACTINOMADURA, ACTINOMYCES, ACTINOPLANES, ACTINOPOLYSPORA, ACTINOSYNNEMA, AGROMYCES, AMORPHOSPORANGIUM, AMPULLARIELLA, ARACHNIA, ARCANOBACTERIUM,
ARTHROBACTER, BREVIBACTERIUM, CASEOBACTER, CELLULOMONAS,
CORYNEBACTERIUM, CURTOBACTERIUM, DACTYLOSPORANGIUM, DERMATOPHILUS, EXCELLOSPORA, FRANKIA, GEODERMATOPHILUS,
INTRASPORANGIUM, KINEOSPORIA, MICROBACTERIUM, MICROBISPORA, MICROMONOSPORA, MICROPOLYSPORA, MICROTETRASPORA,
MYCOBACTERIUM, NOCARDIA, NOCARDIOIDES, NOCARDIOPSIS, OERSKOVIA, PILIMELIA, PLANOBISPORA, PLANOMONOSPORA, PROMICROMONOSPORA, PSEUDONOCARDIA, RENIBACTERIUM, RHODOCOCCUS, ROTHIA, SACCHAROMONOSPORA, SACCHAROPOLYSPORA, SPIRILLOSPORA, SPORICHTHYA, STREPTOALLOTEICHUS, STREPTOMYCES,
STREPTOSPORANGIUM, STREPTOVERTICILLIUM, THERMOMONOSPORA.
[Ecology, isolation, cultivation etc: Book ref. 46, pp. 1915
2123.]
actinomycete Any member of the order ACTINOMYCETALES; the
name is often used to refer specifically to those species which
form mycelium, i.e. excluding many members of the NOCARDIOFORM ACTINOMYCETES.
actinomycetoma See MADUROMYCOSIS.
actinomycin D (actinomycin C1 ) An ANTIBIOTIC from Streptomyces sp; it contains a (red) substituted phenoxazone chromophore linked to two identical pentapeptide lactone rings. All
cell types are potentially susceptible, any resistance being due
to low permeability of cells to the drug. Actinomycin D specifically inhibits DNA-directed RNA synthesis. It binds specifically
to B-DNA as an INTERCALATING AGENT (f ca. 26 ). The phenoxazone chromophore intercalates primarily between two adjacent
(antiparallel) GC pairs, while the lactone rings fit into the minor
groove [ARB (1981) 50 171172]. The drug dissociates from
DNA only very slowly; it blocks the movement of RNA polymerase along its DNA template. (Since actinomycin D shows
little binding to AT-rich PROMOTERS chain initiation is not inhibited.) DNA replication may be insensitive to actinomycin D
because strand separation by the replicative apparatus may facilitate dissociation of the antibiotic.
actinomycosis (1) Any human or animal disease caused by a
species of ACTINOMYCES: A. israelii in man, A. bovis in cattle.
Infection is probably endogenous. Dense nodular lesions are
formed, mainly around the jaw (lumpy jaw), developing into
pus-discharging abscesses. Abscesses may also occur in the
lungs, brain or intestine. Lab. diagnosis: the pathogen may be
isolated from small yellow granules (sulphur granules) present
in the pus. Chemotherapy: e.g. penicillins.
(2) Any human or animal disease caused by an ACTINOMYCETE: e.g. actinomycosis (sense 1); MADUROMYCOSIS. (See
also LACHRYMAL CANALICULITIS.)
actinophage Any BACTERIOPHAGE whose host(s) are member(s)
of the ACTINOMYCETALES. Actinophages, which include both
temperate and virulent types, can be isolated from e.g. soils
and composts; most have a wide host range, but some (e.g.
BACTERIOPHAGE fEC, BACTERIOPHAGE VP5) can infect only one
or a few species. (See also STYLOVIRIDAE). [Soil actinophages
which lyse Streptomyces spp: JGM (1984) 130 26392649.]
Actinophryida An order of protozoa (class HELIOZOEA) in which
the cells have no skeleton and no centroplast (cf. CENTROHELIDA). Some members have flagellated stages. Sexual processes have been observed in some species. Genera include e.g.
ACTINOPHRYS, ACTINOSPHAERIUM, Ciliophrys.
Actinosporangium
acute-phase proteins Various types of protein, found in plasma,
formed as a rapid response to infection; they are synthesized
in the liver e.g. under stimulation from cytokines produced in
a region of INFLAMMATION. These proteins include C-REACTIVE
PROTEIN (CRP) and serum amyloid A (SAA), both of which can
bind to phospholipids in the microbial cell envelope and act as
OPSONINS; additionally, binding by CRP activates COMPLEMENT.
CRP and SAA are so-called pentraxin proteins in which the
molecule consists of five identical subunits.
(See also CD14.)
acute-phase serum Serum obtained from a patient during the
acute phase of a disease.
acute respiratory disease See ARD.
ACV ACYCLOVIR.
ACVs See VACCINE.
acycloguanosine Syn. ACYCLOVIR.
acyclovir (ACV; acycloguanosine; Zovirax) An ANTIVIRAL AGENT,
9-(2-hydroxyethoxymethyl)guanine, which is active against
alphaherpesviruses. It is phosphorylated by the virus-encoded
thymidine kinase to the monophosphate; the monophosphate
is converted by host-cell enzymes to the active triphosphate
form which inhibits DNA polymerase the viral polymerase
being much more sensitive than the cellular a-polymerase. (cf.
BROMOVINYLDEOXYURIDINE.) Uninfected cells do not effectively
phosphorylate acyclovir, and the drug is relatively non-toxic to
the host.
Acyclovir is used topically, systemically or orally in the
treatment of e.g. herpes simplex keratitis, primary genital
herpes, mucocutaneous herpes simplex in immunocompromised
patients, progressive varicella and HERPES ZOSTER. Acyclovir is
not equally active against all alphaherpesviruses its ability to
inhibit the replication of varicella-zoster virus is approximately
10-fold lower than its ability to inhibit replication of herpes
simplex virus. [Use of acyclovir in the treatment of herpes zoster:
RMM (1995) 6 165174 (167170).]
acylalanine antifungal agents See PHENYLAMIDE ANTIFUNGAL
AGENTS.
N-acyl-L-homoserine lactone See QUORUM SENSING.
Acytostelium A genus of cellular slime moulds (class DICTYOSTELIOMYCETES) in which the sorocarp stalk is acellular, cellulosic,
slender, and apparently tubular; no myxamoebae are sacrificed in
stalk formation (cf. DICTYOSTELIUM). The stalk bears a single terminal sorus of spores. Four species are recognized [descriptions
and key: Book ref. 144, pp. 393407].
Ad Human adenovirus: see MASTADENOVIRUS.
AD group ALKALESCENSDISPAR GROUP.
ADA deficiency See ADENOSINE DEAMINASE DEFICIENCY.
ada gene See ADAPTIVE RESPONSE.
adamantanamine See AMANTADINE.
adamantane See AMANTADINE.
Adansonian taxonomy A method of biological classification,
proposed in the 18th century by Michel Adanson, in which
relationships between organisms are defined by the number
of characteristics which the organisms have in common; the
same degree of importance (weighting) is attached to each
characteristic. (cf. NUMERICAL TAXONOMY.)
adaptation Change(s) in an organism, or population of organisms, by means of which the organism(s) become more suited
to prevailing environmental conditions. Genetic adaptation
involves e.g. mutation and selection: those (mutant) organisms in
a given population which are genetically more suited to the existing environment thrive and become numerically dominant. (See
also FLUCTUATION TEST.) Non-genetic (phenotypic) adaptation
cell, their axial filaments arising at the junction between ectoplasm and endoplasm. Asexual reproduction involves plasmotomy. Autogamy occurs when environmental conditions become
unfavourable: the cell produces a gelatinous covering, and many
of its nuclei degenerate; numerous uninucleate daughter cells
are produced, and each encysts. Meiosis within the cyst results
in two haploid gametes which fuse, and the resulting zygote
remains dormant until conditions improve.
Actinosporangium See STREPTOMYCES.
Actinosporea A class of protozoa (phylum MYXOZOA) which
are parasitic in invertebrates (particularly annelid worms). The
spores contain 3 polar capsules (each enclosing a single polar filament) and several to many sporoplasms. The spore wall consists
of 3 valves which may be smooth (e.g. in Sphaeractinomyxon) or
drawn out into long, horn-like processes (as in Triactinomyxon,
a parasite of tubificid and sipunculid worms). (cf. WHIRLING DISEASE.)
Actinosynnema A genus of bacteria (order ACTINOMYCETALES,
wall type III) which occur e.g. on vegetable matter in aquatic
habitats. The organisms form a thin, branching, yellow substrate
mycelium (hyphae <1 m diam.) on which develop synnemata
(up to ca. 180 m in height) or dome-like bodies; aerial hyphae
may arise from the substrate mycelium, or from the tips of the
synnemata, and give rise to chains of spores which become
motile (flagellated) in liquid media. GC%: ca. 71. Type species:
A. mirum. [Book ref. 73, pp 116117.]
activated acetic acid pathway See AUTOTROPH.
activated sludge See SEWAGE TREATMENT.
activation (immunol.) (1) (of lymphocytes) A process which
begins with BLAST TRANSFORMATION and continues with proliferation (cell division) and differentiation; some authors use
activation to refer specifically to stage(s) preceding proliferation. (2) (of complement) See COMPLEMENT FIXATION. (3) See
MACROPHAGE. (4) (of spores) See ENDOSPORE and SPORE.
activation-induced cytidine deaminase See RNA EDITING.
activator (1) Syn. COFACTOR (sense 2). (2) See SPORE. (3) See
OPERON and REGULON.
active bud See LIPOMYCES.
active immunity Specific IMMUNITY (3) afforded by the bodys
own immunological defence mechanisms following exposure to
antigen. (cf. PASSIVE IMMUNITY.)
active immunization See IMMUNIZATION.
active transport See TRANSPORT SYSTEMS.
actomyosin An actinmyosin complex (see ACTIN and MYOSIN).
aculeacin A An antibiotic which is active against yeasts, inhibiting the formation of yeast CELL WALL glucan. Echinocandin B is
a structurally related antibiotic with an apparently similar mode
of action. (cf. PAPULACANDIN B.)
aculeate Slender and sharp-pointed, or bearing narrow spines.
acute (med.) Refers to any disease which has a rapid onset
and which persists for a relatively short period of time (e.g.
days) terminating in recovery or death. The term is also used
to refer to an exceptionally severe or painful condition. (cf.
CHRONIC.)
acute cardiac beriberi See CITREOVIRIDIN.
acute haemorrhagic conjunctivitis (AHC) A highly infectious
form of CONJUNCTIVITIS, a worldwide pandemic of which
occurred during 19691971; it is caused by enterovirus 70 (see
ENTEROVIRUS) and is characterized by subconjunctival haemorrhages ranging from petechiae to larger areas covering the bulbar
conjunctivae. Recovery is usually complete in ca. 10 days.
acute herpetic gingivostomatitis See GINGIVITIS.
acute necrotizing ulcerative gingivitis See GINGIVITIS.
10
Adenoviridae
Adeleina A suborder of protozoa (order Eucoccida [JP (1964) 11
720] or Eucoccidiida [JP (1980) 27 3758]) equivalent to the
ADELEORINA.
Adeleorina A suborder of protozoa (order EUCOCCIDIORIDA)
in which syzygy characteristically occurs (cf. EIMERIORINA,
HAEMOSPORORINA). Genera include Adelea, Haemogregarina,
Klossiella.
adenine arabinoside Syn. VIDARABINE.
adenitis Inflammation of gland(s).
adeno-associated viruses See DEPENDOVIRUS.
adeno-satellite viruses See DEPENDOVIRUS.
adenosine See NUCLEOSIDE and Appendix V(a).
adenosine 3 , 5 -cyclic monophosphate See CYCLIC AMP.
adenosine deaminase deficiency A congenital lack of the
enzyme adenosine deaminase (EC 3.5.4.4), the effects of which
include a marked reduction in the numbers of functional B and
T lymphocytes. (See SEVERE COMBINED IMMUNODEFICIENCY.)
The disease has been treated by GENE THERAPY.
adenosine triphosphatase See ATPASE.
adenosine 5 -triphosphate See ATP.
Adenoviridae (adenovirus family) A family of non-enveloped,
icosahedral, linear dsDNA-containing viruses which infect mammals (genus Mastadenovirus) or birds (genus Aviadenovirus).
Adenoviruses are generally specific for one or a few closely
related host species; infection may be asymptomatic or may
result in various diseases (see AVIADENOVIRUS and MASTADENOVIRUS). Many adenoviruses can induce tumours when injected
into newborn rodents, but none is known to cause tumours
in natural circumstances. In cell cultures, adenoviruses cause
characteristic CPE, including the rounding of cells and the formation of grape-like clusters of cells; adenovirus replication and
assembly occur in the nucleus, resulting in the formation of
intranuclear inclusion bodies. Virions sometimes form paracrystalline arrays. Many adenoviruses can haemagglutinate RBCs
from various species.
The adenovirus virion consists of an icosahedral CAPSID (ca.
7090 nm diam.) enclosing a core in which the DNA genome
is closely associated with a basic (arginine-rich) viral polypeptide (VP), VII. The capsid is composed of 252 capsomers: 240
hexons (capsomers each surrounded by 6 other capsomers) and
12 pentons (one at each vertex, each surrounded by 5 peripentonal hexons). Each penton consists of a penton base (composed
of viral polypeptide III) associated apparently by hydrophobic interactions with one (in mammalian adenoviruses) or two
(in most avian adenoviruses) glycoprotein fibres (viral polypeptide IV); each fibre carries a terminal knob ca. 4 nm in diam.
The fibres can act as haemagglutinins and are the sites of attachment of the virion to a host cell-surface receptor. The hexons
each consist of three molecules of viral polypeptide II; they
make up the bulk of the icosahedron. Various other minor viral
polypeptides occur in the virion.
The adenovirus dsDNA genome (MWt ca. 2025 106 for
mammalian strains, ca. 30 106 for avian strains) is covalently
linked at the 5 end of each strand to a hydrophobic terminal
protein, TP (MWt ca. 55000); the DNA has an inverted terminal
repeat (ITR) of different length in different adenoviruses. In most
adenoviruses examined, the 5 -terminal residue is dCMP (dGMP
in CELO virus).
Adenovirus virions are stable and are not inactivated by e.g.
lipid solvents or by pancreatic proteases, low pH, or bile salts.
Replication cycle. The virion attaches via its fibres to a
specific cell-surface receptor, and enters the cell by endocytosis
or by direct penetration of the plasma membrane. Most of
adenoviruses
effects on various metabolic processes the activity of certain
enzymes being regulated by the actual concentration of a given
adenine nucleotide or by the ratio of particular nucleotides
(e.g. ATP:ADP). Thus, e.g., in certain yeasts the enzyme
phosphofructokinase is inhibited by ATP (an effect which is
reversed by AMP), while in Escherichia coli the same enzyme
is stimulated by ADP; hence, glycolysis tends to be stimulated
when the EC is depressed.
Energy charge is also a regulatory factor for the degree of
supercoiling (superhelical density) in a cells DNA; changes in
superhelical density can, in turn, influence the activity of various
gene promoters. Thus, via energy charge and superhelicity,
the environment can modulate the expression of particular
genes. (Interestingly, the expression of genes or operons may
also be regulated by local changes in superhelicity due to
divergent transcription from closely spaced gene promoters
[Mol. Microbiol. (2001) 39 11091115].)
Estimations of EC involve both rapid sampling and precautions to prevent hydrolysis or interconversion of adenine
nucleotides. ATP is often measured by techniques which involve
CHEMILUMINESCENCE.
adenylate kinase An enzyme (EC 2.7.4.3) which catalyses
the reversible conversion of two molecules of adenosine
5 -diphosphate (ADP) to one molecule each of ATP and AMP.
[Structural and catalytic properties of adenylate kinase from
Escherichia coli: JBC (1987) 262 622629.]
adenylylsulphate See APS.
ADH ARGININE DIHYDROLASE.
adherent cells (immunol.) Cells which adhere to e.g. glass and
plastics; they include e.g. MACROPHAGES and DENDRITIC CELLS.
adhesin A cell-surface component, or appendage, which mediates ADHESION to other cells or to inanimate surfaces or interfaces; there are many different types of adhesin, and a given
organism may have more than one type. (The term adhesin is
also used to include certain secreted substances which behave
as adhesins e.g. MUTAN.)
Bacterial adhesins. Many bacterial adhesins are FIMBRIAE,
and in some pathogenic species fimbrial adhesins are important virulence factors which mediate the initial stage of pathogenesis (adhesion to specific site(s) in the host organism).
For example, fimbria-mediated adhesion is important for virulence in ETEC strains of Escherichia coli whose capacity to
cause disease depends on their ability to bind to the intestinal mucosa; among strains of ETEC there are more than 10
different types of fimbrial adhesin (as well as non-fimbrial
adhesins) [RMM (1996) 7 165177]. [Expression of fimbriae
by enteric pathogens (review): TIM (1998) 6 282287.] Fimbrial adhesins are also important in Haemophilus influenzae type
b for the initial binding to respiratory tract epithelium [adhesins
in Haemophilus, Actinobacillus and Pasteurella: FEMS Reviews
(1998) 22 4559]. (See also UPEC and P FIMBRIAE.)
Some fimbrial adhesins additionally function as an INVASIN
(see e.g. UPEC) or as a phage receptor (see e.g. BACTERIOPHAGE
CTX8).
The dimensions and charge characteristics of fimbriae are such
that they experience minimal repulsion from a surface bearing
charge of the same polarity; thus, fimbrial adhesins can help to
bridge the gap between the charged bacterial surface (see ZETA
POTENTIAL) and the surface of another cell or substratum which
bears a charge similar (in polarity) to that on the bacterium.
Non-fimbrial adhesins include the filamentous haemagglutinin (FHA) of Bordetella pertussis, the high-molecular-weight
adhesion proteins (HMW1, HMW2) of non-typable strains of
adiaspore
bonding, and van der Waals forces. Because some types
of cell resemble colloids in their dimensions and electrical
characteristics (see ZETA POTENTIAL), the interaction between a
cell and a substratum (or between two cells) in an aqueous
medium is sometimes considered in the context of classical
colloid theory in particular the theory of Derjaguin, Landau,
Verwey and Overbeek (the DLVO theory). The DLVO theory
supposes that a particle which bears a distributed surface
charge of given polarity is surrounded by a layer of ions of
opposite charge forming a so-called double layer extending
some distance from the surface of the particle; two similarly
charged particles will therefore be mutually repulsive through
the interaction of their double layers. An increase in the
ionic concentration in the medium effectively compresses each
double layer so that the particles can then approach each
other more closely; in a number of cases, cellsubstratum or
cellcell contact has been shown to be facilitated by raising
the concentration of electrolyte. However, a rigid application of
the DLVO theory (or any other mathematically based theory) to
biological systems is made difficult by a number of factors which
include the susceptibility of the cell to physical deformation, the
chemical complexity and non-uniformity of the cell surface, and
the possibility of ionic flux across juxtaposed surfaces.
Microorganisms which are normally attached to a substratum
may be dispersed by means of either non-adherent progeny
or propagules or they may be able to detach, temporarily,
in order to colonize fresh surfaces. The hydrophobic, benthic
cyanobacterium Phormidium J-1 appears to achieve dispersal
by forming an emulsifying agent (EMULCYAN) which masks cellsurface hydrophobicity permitting detachment; the emulcyan
is presumed to be washed off the cells at some stage so that
attachment is again possible [FEMS Ecol. (1985) 31 39].
adhesion site (Bayers junction; Bayers patch) In Gram-negative bacteria: a localized fusion between the OUTER MEMBRANE
and CYTOPLASMIC MEMBRANE [Book ref. 101, pp. 167202]. In
electronmicrographs, a plasmolysed cell may show adhesion
sites under some experimental conditions but not under others
[JB (1984) 160 143152]. [Cell envelope fraction with apparent
adhesion sites: JBC (1986) 261 428443.]
Adhesion sites appear to be osmotically sensitive, physiologically important regions of the cell envelope which serve e.g. as
sites for the export of proteins (such as porins), LPS molecules
[JB (1982) 149 758767] and filamentous phages, as sites of
infection for certain phages, and as the anchorage sites of e.g.
F pili. Certain proteins (e.g. penicillin binding protein 3, THIOREDOXIN [JB (1987) 169 26592666]) have been associated with
adhesion sites.
[Mol. Microbiol. (1994) 14 597607.]
(See also PERISEPTAL ANNULUS, and lysis protein in LEVIVIRIDAE.)
adiaspiromycosis (adiaspirosis; haplomycosis) A non-infectious
MYCOSIS which primarily affects animals, rarely affecting
man. It is caused by Chrysosporium parvum var. parvum
(formerly Emmonsia parva or Haplosporangium parvum) or by
C. parvum var. crescens (formerly E. crescens). Infection occurs
by inhalation of conidia (formed e.g. in soil); the conidia enlarge
within the lungs to reach diameters of ca. 40 m (var. parvum)
or 400 m (var. crescens). Granulomas may develop around the
adiaspores.
adiaspirosis Syn. ADIASPIROMYCOSIS.
adiaspore A spore (conidium) which grows in size without
dividing see e.g. ADIASPIROMYCOSIS and CHRYSOSPORIUM.
adjuvant
In the carrier state the incidence of ATL is low; latency can
last for many decades.
The disease has been categorized into four clinical subtypes: acute, chronic, smouldering and lymphoma. Acute cases
comprise the majority. Chronic and smouldering forms often
progress to the acute form. In some cases disease is nodal rather
than leukaemic.
Various manifestations of ATL may be seen. In many cases
there are lesions in liver, spleen and/or lymph nodes, though
other sites (including the central nervous system) may be
affected; skin lesions may include nodules, ulcers or rashes.
Hypercalcaemia may be present, and the undermined immune
system may permit infection by opportunist pathogens (e.g.
Pneumocystis carinii, cytomegalovirus).
Leukaemic cells are monoclonal, originating from a single cell
infected with HTLV-I; the cells are larger than normal and may
have multilobed or convoluted nuclei.
The median survival time for the acute form of ATL is
reported to be 6 months (2 years for the chronic form).
Lab. diagnosis. Diagnosis involves e.g. clinical observation,
serology (for anti-HTLV-I antibody) and detection of abnormal
T cells by microscopy.
Chemotherapy. Given the absence of standard therapy, it
has been recommended that treatment be limited to acute and
lymphoma-type cases; for these patients combination chemotherapy may be successful, but relapses (often involving the CNS)
are common.
[ATL (epidemiology, leukaemogenesis, clinical features, laboratory findings, diagnosis, treatment, prognosis and prevention):
BCH (2000) 13 231243.]
adjuvant (1) (immunol.) Any substance which, when administered with or before an antigen, heightens and/or affects qualitatively the immune response in terms of antibody formation
and/or the cell-mediated response. (The adjuvant L18-MDP(A)
has also been reported to enhance non-specific phagocytosis by
polymorphonuclear leucocytes [JGM (1982) 128 23612370].)
Adjuvants include e.g. BCG, aluminium hydroxide, and waterin-oil emulsions (e.g. FREUNDS ADJUVANT). (2) Any substance
which is added to a drug or other chemical (e.g. a disinfectant)
to enhance its activity.
Adjuvant 65 A water-in-oil emulsion ADJUVANT made by emulsifying peanut oil with mannide monooleate and stabilizing with
aluminium monostearate.
adk gene (dnaW gene) In Escherichia coli: the gene for adenylate
kinase.
Adler test A test used for the identification of Leishmania
spp. The organisms are cultured in an immune serum; in the
presence of homologous antibodies, promastigotes develop in
clusters or syncytia.
adnate (1) Of the region of lamellastipe attachment in an
agaric: extending for a length equal to much or most of the
depth of the lamella.
(2) Of flagellar spines: flattened against the flagellum from
which they arise.
adnexed (mycol.) Of the region of lamellastipe attachment in
an agaric: extending for a length equal to only a small fraction
of the depth of the lamella.
adonitol Syn. RIBITOL.
adoptive immunity Syn. PASSIVE IMMUNITY.
adoral ciliary spiral See AZM.
adoral zone of membranelles See AZM.
ADP Adenosine 5 -diphosphate. (See also ATP and ADENYLATE
KINASE.)
ADP-ribosylation The transfer of an ADP-ribosyl group
from NAD+ to a protein, catalysed by an ADP-ribosyl
transferase. In eukaryotic cells, various proteins may be
ADP-ribosylated apparently as a normal regulatory mechanism; certain bacterial toxins act by exerting an ADP-ribosyl
transferase function: see e.g. BOTULINUM C2 TOXIN, CHOLERA
TOXIN, DIPHTHERIA TOXIN, EXOTOXIN A and PERTUSSIS TOXIN. ADPribosylation also occurs e.g. in cells of Escherichia coli infected
with BACTERIOPHAGE T4, the host RNA polymerase undergoing phage-induced ADP-ribosylation. [Review: TIBS (1986) 11
171175.]
adrenalin (epinephrine) A multifunctional hormone, secreted by
the adrenal gland, which affects e.g. carbohydrate metabolism
and the activity of smooth muscle, particularly that of the
cardiovascular and bronchial systems. Adrenalin is used e.g. for
the treatment of ANAPHYLACTIC SHOCK in which it counteracts
the effects of histamine, relaxing smooth muscle and reducing
vascular permeability.
adriamycin See ANTHRACYCLINE ANTIBIOTICS.
ADRY reagents Certain substituted thiophenes which can e.g.
stimulate the photooxidation of cytochrome b559 in photosystem
II (see PHOTOSYNTHESIS).
adsorption (serol.) Non-specific adherence of substances (in
solution or in suspension) to cells or to other forms of particulate
matter. (See e.g. BOYDEN PROCEDURE; cf. ABSORPTION.)
adsorption chromatography See CHROMATOGRAPHY.
adult T-cell leukaemia (ATL; adult T-cell leukaemia/lymphoma,
ATLL) A T-cell LEUKAEMIA (q.v.) which affects adults; the
causal agent is an exogenous retrovirus, HTLV-I (see HTLV). ATL
is endemic in certain regions of Japan, the Caribbean, Africa and
the Americas.
14
aesculin
at 5 C. Three subspecies are recognized. Subsp salmonicida is
indole ve, aesculin +ve, and produces a water-soluble brown
pigment when grown aerobically on media containing 0.1% tyrosine or phenylalanine. Subsp achromogenes is indole +ve/ve,
aesculin ve, and does not produce brown pigment. Subsp
masoucida is indole +ve, aesculin +ve, and does not produce
brown pigment. A. salmonicida is haemolytic on blood agar.
The species is strictly parasitic and often pathogenic in fish,
causing e.g. FURUNCULOSIS and secondary infections in various
other diseases.
[Aeromonas bacteriophages: Ann. Vir. (1985) 136E 175199.]
aerosol Minute (colloidal) particles of liquid and/or solid dispersed in a gas (e.g. air), formed e.g. by sneezing, coughing,
liquids splashing, bubbles bursting, etc. An aerosol may contain
viable microorganisms.
aerotaxis A TAXIS in which a (motile) cell migrates along
an oxygen concentration gradient to a location where the
concentration of oxygen is optimal for that cell.
In bacteria, aerotaxis appears to be exhibited by all aerobic
and facultatively aerobic motile species. Interestingly, though,
organisms which use oxygen as terminal electron acceptor in
energy metabolism do not necessarily migrate to positions where
oxygen is at atmospheric levels; for example, the respiratorytype bacterium Azospirillum brasiliense is microaerophilic, and
this organism migrates towards regions where the oxygen
concentration is only 35 M. (This species may have a highly
efficient oxidase which enables it to carry out oxygen-based
respiratory metabolism in microaerobic conditions.)
For some time it has been thought that aerotaxis may be linked
to changes in proton motive force (pmf). In support of this idea,
it was found that different types of change in pmf (i.e. increases
or decreases) are associated with different effects on motility;
thus, for example, if the partial pressure of oxygen is kept
constant, then an artificially induced increase in pmf encourages
smooth, continual swimming, while a decrease in pmf promotes
tumbling in peritrichously flagellated cells. More recently it
has been shown that, in A. brasiliense, pmf increases when the
cell swims towards the preferred concentration of oxygen and
decreases when the cell swims in the opposite direction; this has
suggested that the change in level of pmf acts as a signal which
regulates aerotactic movements [JB (1996) 178 51995204].
Aerotaxis apparently cannot occur in a bacterium in which the
pmf is at a maximum; under such conditions certain other (pmfindependent) taxes e.g. CHEMOTAXIS may occur.
In Escherichia coli a sensor protein, Aer, may mediate
aerotaxis by responding to redox changes in component(s) of the
electron transport chain; the Tsr protein (an MCP in chemotaxis)
appears to be another, independent sensor for aerotaxis and may
respond to changes in pmf [PNAS (1997) 94 1054110546].
aerotolerant Refers to an ANAEROBE which, in the presence of
air, can either survive (but not grow) or grow at sub-optimal
rates.
aeruginocin Syn. PYOCIN.
aesculin (esculin) The 6-b-D-glucosyl derivative of 6,7-dihydroxycoumarin. Certain bacteria (e.g. most strains of the
former group D streptococci, many Bacteroides spp including
B. fragilis) can hydrolyse aesculin to yield 6,7-dihydroxycoumarin which gives a brown coloration with soluble ferric salts.
(Hydrolysis may also be detected by the disappearance of
aesculin fluorescence under Woods lamp.)
Various media are used for aesculin hydrolysis tests. Aesculin
broth may contain e.g. aesculin (0.1%) and FeCl3 (0.05%) in
heart infusion broth. Aesculin agar is aesculin broth gelled with
aethalium
nucleotides (a-[33 P]-dATP) that are incorporated into products
during amplification [BioTechniques (2000) 28 622623].)
[Taxonomic evaluation of Bacillus anthracis and related
species by AFLP fingerprinting: JB (1997) 179 818824.
AFLP fingerprinting used for detecting genetic variation in
Xanthomonas: Microbiology (1999) 145 107114. AFLP-based
study of Escherichia coli : JCM (1999) 37 12741279. Review
of AFLP fingerprinting: JCM (1999) 37 30833091.]
African farcy Syn. EPIZOOTIC LYMPHANGITIS.
African horse sickness An infectious HORSE DISEASE caused by
an Orbivirus and transmitted by insects (e.g. Culicoides spp); it
occurs in Africa, parts of the Middle East, and the Mediterranean
region. The disease may be acute, with an incubation period
of ca. 57 days, followed by fever, laboured breathing, severe
paroxysms of coughing, and a profuse nasal discharge of
yellowish, frothy serous fluid; death usually occurs within 45
days of onset. Subacute forms of the disease may occur in
enzootic areas: an incubation period of up to 3 weeks is followed
by oedema of the head region, spreading to the chest; cardiac
and pulmonary symptoms and paralysis of the oesophagus may
occur, but mortality rates are generally lower than in the acute
form. A mild form involving fever and moderate dyspnoea
(horse sickness fever) may occur e.g. in partially immune
animals. African horse sickness may also cause severe debility in
mules and donkeys, but mortality rates are lower than in horses.
Control: e.g. vaccination; control of vectors.
African swine fever A highly infectious PIG DISEASE which
clinically resembles European SWINE FEVER (q.v.); it occurs e.g.
in Africa, Spain and Portugal. The causal agent is a virus
previously classified in the IRIDOVIRIDAE but currently considered
to belong to a separate family. The virion is icosahedral,
enveloped, and contains a DNA-dependent RNA polymerase
and RNA-modifying enzymes; the genome is dsDNA (MWt ca.
100 106 ) in which the strands are covalently joined at each end
(cf. POXVIRIDAE), and which contains terminal inverted repeats.
African trypanosomiases See TRYPANOSOMIASIS.
ag (immunol.) ANTIGEN.
Agamococcidiorida An order in the COCCIDIASINA.
agamont See ALTERNATION OF GENERATIONS.
agar A complex galactan which is widely used (in gel form) as
a base for many kinds of solid and semi-solid microbiological
MEDIUM; agar (or agarose see below) is also used e.g. in techniques such as GEL DIFFUSION, GEL FILTRATION and ELECTROPHORESIS, and in industry as a gelling agent in foods, pharmaceuticals
etc. Agar is produced by many marine rhodophycean algae and is
obtained commercially from e.g. Gelidium and Gracilaria spp;
in the alga it is associated with the CELL WALL and intercellular matrix. (The term agar derives from the Malay agar-agar
which refers to certain edible seaweeds.)
Agar consists of two main components: agarose (ca. 70%) and
agaropectin (ca. 30%). Agarose is a non-sulphated linear polymer consisting of alternating residues of D-galactose and 3,6anhydro-L-galactose: [-3,6-anhydro-a-L-galactopyranosyl-(1
3)-b-D-galactopyranosyl-(1 4)-]n ; in agarose from some species, a proportion of the D-galactose residues have 6-O-methyl
substituents. Agaropectin is a mixture of sulphated galactans which may also contain e.g. glucuronic acid or pyruvic
acid, depending on source. (Agar-like substances from noncommercial seaweeds show various structural differences from
commercial agar [Book ref. 38, pp. 291292].)
An agar gel is a translucent or transparent jelly-like substance formed when a mixture of agar and water is heated
to >100 C and then cooled; gelling occurs at ca. 4045 C.
(a)
(b)
adaptor
restriction fragment
NNNG3
adaptor
5AATTGNNNNNNN3
NNNCTTAA5
(c)
CNNNNNNN5
NNNGAATTGNNNNNNN3
NNNCTTAACNNNNNNN5
(d)
NNNGAATTGNNNNNNN3
TCTTAACNNNNNNN5
primer
17
AHG
Agrobacterium spp occur in soil, mainly in the rhizosphere.
All (except A. radiobacter) can infect a wide range of dicotyledonous plants (and some gymnosperms) and induce the formation of self-proliferating galls or adventitious roots. The
species are defined primarily or solely on the basis of their
pathogenic characteristics: A. radiobacter is non-pathogenic,
A. rhizogenes causes HAIRY ROOT, A. rubi causes CANE GALL,
and A. tumefaciens causes CROWN GALL. However, pathogenicity depends on the presence of a plasmid(s) and can readily
be altered or lost; hence the currently recognized species do
not reflect true taxonomic relationships among the agrobacteria.
[Book ref. 22, pp. 244254.]
[Media and culture: Book ref. 45, 842855.]
agrocin 84 See AGROCINS.
agrocinopines A class of (sugar phosphodiester) opines found in
CROWN GALL. (See also AGROCINS.)
agrocins Antibiotics which are produced by certain strains of
Agrobacterium and which are active against other strains of
the same genus; being non-protein in structure, agrocins are
not strictly BACTERIOCINS. Agrocin 84 is produced by a nonpathogenic, nopaline-catabolizing strain of A. radiobacter (strain
84, NCPPB 2407) and is selectively active against agrobacteria which harbour a nopaline Ti plasmid. Strain 84 is used
in the BIOLOGICAL CONTROL of CROWN GALL; a cell suspension
is used to treat seeds, roots or wounded plant surfaces (e.g.
graft wounds), and almost 100% control of nopaline pathogens
(responsible for most of the economic damage due to crown
gall) can be achieved. Agrocin 84 is an adenine nucleotide
derivative containing an N 6 -phosphoramidate substituent (necessary for uptake by sensitive cells) and a 5 -phosphoramidate
substituent (necessary for toxicity). Agrocin 84 is taken up by
sensitive strains via a high-affinity agrocin permease, apparently an agrocinopine transport system normally inducible by
agrocinopines (sugar phosphodiesters) present in galls caused by
nopaline strains. Strain 84 contains at least three plasmids: one
(pAgK84, 47.7 kb) coding for agrocin 84 production, another
(pAt84b, ca. 200 kb) coding for nopaline catabolism. pAgK84
is self-transmissible only at very low frequencies, but can be
mobilized by the conjugative plasmid pAt84b. As transfer of
pAgK84 to a crown gall pathogen could threaten the continued use of agrocin 84 in biocontrol, a transfer-deficient mutant
strain was prepared. However, strain K84 apparently exerts some
activity against agrocin 84-resistant pathogens independently of
pAgK84 [AEM (1999) 65 19361940].
Agrocybe See AGARICALES (Bolbitiaceae).
agroinfection A method for introducing viral DNA (or cDNA)
into a plant. Viral DNA is initially incorporated into the T-DNA
part of a Ti plasmid. The plasmid is then introduced into the
bacterium Agrobacterium tumefacienswhich is used to infect
the plant; during infection the viral DNA is transferred to plant
cells within the T-DNA (see CROWN GALL). [Example of use: JV
(2003) 77 32473256.]
Agromyces A genus of microaerophilic to anaerobic, catalasenegative, asporogenous bacteria (order ACTINOMYCETALES, wall
type VII see also PEPTIDOGLYCAN). The organisms grow as a
branched mycelium which subsequently fragments into coccoid
and diphtheriod forms; metabolism: oxidative. A. ramosus, the
type species, occurs in large numbers in certain soils; it appears
to attack and destroy other species of bacteria [AEM (1983) 46
881888].
agropine See CROWN GALL and HAIRY ROOT.
Agropyron mosaic virus See POTYVIRUSES.
AHG (serol.) Anti-human globulin: ANTIGLOBULIN homologous
to human globulins.
AHL
Antibodies (e.g. anti-gp120, anti-p24) are first detectable
612 weeks after infection; their appearance may follow, or
coincide with, the rapid decline in viraemia.
During seroconversion some patients experience a seroconversion illness which may include e.g. fever, sore throat, skin
rash, generalized lymphadenopathy, pneumonitis, gastrointestinal and/or CNS involvement.
A subsequent phase of infection is characterized by persistent generalized lymphadenopathy (PGL) (also called lymphadenopathy syndrome) swollen lymph nodes reflecting an
active immune response to HIV. (In some cases, PGL is the
first manifestation of disease following infection, i.e. in patients
who do not exhibit an acute phase.) Infection may then become
asymptomatic (clinically latent), and this state may continue for
months or years (during which time viral replication continues).
Patients with clinically latent infection, as well as those
with PGL, may pass directly to AIDS. Alternatively, both
types of patient may progress to AIDS via a further stage
commonly referred to as the AIDS-related complex (ARC)
(= category B of the CDC clinical staging system). Category B
diseases include bacillary angiomatosis (see BARTONELLA),
oropharyngeal candidiasis, HAIRY LEUKOPLAKIA, LISTERIOSIS, PID
(pelvic inflammatory disease), herpes zoster (involving at least
two distinct episodes, or more than one dermatome), and peripheral neuropathy.
In AIDS, the final stage, the CD4+ count is often
<200 cells/ml; there is high-level viraemia, and the p24 antigen
is again detectable. Note that the AIDS-defining diseases (see
above) include those that result from infection by low-grade
pathogens, i.e. organisms which generally cause disease only
in those patients who are severely immunodeficient (including
HIV individuals who may be immunodeficient for other
reasons). Conversely, the high-grade pathogens (which can
cause disease even in the immunocompetent) may cause disease
in HIV+ patients whose immune system is only marginally
impaired.
Immunopathogenesis.
In HIV+ individuals, the reduction in numbers of CD4+ T cells
may arise in various ways e.g. (i) productive infection by HIV
and subsequent lysis; (ii) killing of HIV-infected cells by HIVspecific CD8+ cytotoxic T cells (see T LYMPHOCYTE) or by NK
CELLS; (iii) ADCC (of virus-infected cells). It also appears that
non-infected CD4+ T cells may be susceptible to attack e.g.
by HIV-specific cytotoxic T cells or by NK CELLS; this may
occur when free (isolated) gp120 protein (see HIV) binds to
CD4 on virus-free (bystander) cells such cells then becoming
vulnerable to the antiviral immune response. CD4+ cells may
also be vulnerable to APOPTOSIS if viral gp120 cross-links CD4
molecules on the cell surface, such cross-linking resulting in an
upregulation of the FAS antigen.
Following depletion of CD4+ T cells, the virus may persist
within tissue macrophages (see under Chemotherapy, below).
HIV infection produces (i) a direct effect (death of infected
cells), and (ii) an indirect effect (weakening of the overall
immune system). The direct effect may include neurological
deficits (e.g. encephalopathy) as well as immunological damage;
the indirect effect is manifested in the range of ARC and AIDSdefining diseases (including both neoplastic and opportunistic
diseases).
Depletion of CD4+ T cells is only one of many abnormalities
in the immune system of HIV+ /AIDS patients. Other types of
cell (including B cells) are reported to display abnormalities, and
DELAYED HYPERSENSITIVITY reactions may be either absent or of
reduced intensity.
air
The role of CYTOKINES in HIV infection has yet to be clarified,
but it seems that, at some stage, the cytokine milieu becomes
aberrant, and that increased amounts of e.g. TNF-a and several
interleukins (including INTERLEUKIN-4) are formed. It has been
suggested that TNF-a may promote viral transcription through
activation of the host cells nuclear transcription factor, NFkB (see HIV), and that increased levels of IL-4 may bring
about a (deleterious) switch to the Th2 subset of T cells (see
T LYMPHOCYTE).
Diagnosis of HIV infection.
In adults and adolescents, laboratory diagnosis of HIV infection
is serologically based.
The viral antigen p24 (major core protein) is commonly
detectable (transiently) in blood during the initial viraemic
(acute) phase of infection, i.e. before any antibodies are
detectable. However, not all patients exhibit an acute phase of
infection; while a positive test for p24 is useful, a negative test
is not a reliable indication of the absence of HIV infection.
Tests for anti-HIV antibodies (e.g. anti-gp120) may be carried out e.g. by ELISA. A positive result may be confirmed by
Western blot analysis of viral proteins. Antibodies are commonly
present by 6 weeks post-infection, although positive serology
is sometimes delayed. (In some cases, patients who are serologically negative have been implicated, epidemiologically, in the
transmission of AIDS.)
Serology is inappropriate for neonates and very young children: if the mother is HIV+ then, owing to passive transfer of
maternal antibodies, the neonate will also contain anti-HIV antibodies, whether infected or not. Culture is a useful approach for
diagnosis in this context.
The pre-seroconversion window (the period, post-infection,
before development of antibodies) presents a problem in blood
transfusion because donor samples taken in this period are likely
to contain virus. To minimize this risk, samples can be subjected
to PCR-based tests designed to detect viral nucleic acid. Such tests
may involve initial concentration of virions from plasma [Lancet
(1999) 353 359363]. Alternatively, the procedure may test for
the integrated (i.e. provirus) form of HIV; in this case, PCR
is carried out on DNA extracted from blood leukocytes [PNAS
(1999) 96 63946399]. (See also BLOOD DNA ISOLATION KITS.)
Chemotherapy for HIV infection.
The drug zidovudine (see AZT) was the first agent used for
the treatment of HIV infection. Although initially successful,
the use of AZT was found to be limited by the development
of drug-resistant strains of HIV. In recent years, combinations
of ANTIRETROVIRAL AGENTS have been used in so-called highly
active antiretroviral therapy (see HAART). Attempts are being
made to extend the range of antiretroviral agents by developing
inhibitors of the viral integrase (in order to inhibit integration of
HIV provirus into the host cells genome). (See also NU-1320.)
Even with HAART, however, HIV commonly (or always)
emerges after cessation of therapy, and it is generally believed
that, during therapy, HIV persists in CD4+ memory T cells.
However, using a chimeric virus (simian immunodeficiency
virus/HIV-1), it has been shown that tissue macrophages (in
lymph nodes, liver, spleen etc.) form the principal reservoir of
virus following depletion of CD4+ T cells in rhesus macaques;
this has suggested that macrophages may be a major source of
HIV in the symptomatic phase of human infection [PNAS (2001)
98 658663].
The drug nevirapine is reported to inhibit intrauterine transmission of HIV to the fetus in a proportion of cases.
One problem associated with chemotherapy is that the combination of drugs used in HAART is often augmented by other
air bladder
apparently functions as an overwintering propagule. Akinetes are
formed under various growth-limiting environmental conditions
(e.g., nutrient limitation); in e.g. Anabaena spp, akinetes develop
adjacent to HETEROCYSTS, while in e.g. Nostoc spp they develop
in positions midway between two heterocysts. An akinete is
typically larger than a vegetative cell; it has a thickened wall
and granular cytoplasm rich in storage materials (cyanophycin,
glycogen etc). Rates of photosynthesis, respiration etc are
usually much lower in akinetes than in vegetative cells; in
e.g. Anabaena doliolum, akinetes appear to be deficient in both
photosynthesis and inorganic nitrogen metabolism [JGM (1984)
130 12991302]. On germination of an akinete, a single cell
or short filament may be released via a pore in or by rupture
of the akinete wall, depending on species.
(2) (algol.) A thick-walled non-motile resting cell produced
by certain algae of the CHLOROPHYTA and XANTHOPHYCEAE.
(3) (mycol.) A non-motile spore.
akinetoplasty Obsolete syn. DYSKINETOPLASTY.
AktA (of Actinobacillus actinomycetemcomitans) See RTX TOXINS.
AKV A replication-competent MURINE LEUKAEMIA VIRUS which
occurs endogenously in various strains of mice (e.g. AKR,
BALB/c). It appears to have given rise to the transforming
virus AKR mink cell focus-forming virus (AKR-MCF) by
recombination with one or more endogenous xenotropic viruses.
(See also MCF VIRUSES.)
alafosfalin (alaphosphin; L-alanyl-L-1-aminoethylphosphonic acid)
A synthetic ANTIBIOTIC which is taken up by the LL-dipeptide
transport system of a sensitive cell; it is subsequently hydrolysed
intracellularly to release the inhibitory component, 1-aminoethylphosphonic acid (ala-P), which itself cannot cross the
cytoplasmic membrane. (cf. WARHEAD DELIVERY.) Ala-P acts
by competitively inhibiting alanine racemase and at higher
concentrations by inhibiting the addition of L-alanine to UDPMurNAc during PEPTIDOGLYCAN synthesis. Alafosfalin has a
broad spectrum of activity, but is generally more effective against
Gram-negative than Gram-positive bacteria.
alamethicin A water-soluble peptide antibiotic (MWt ca. 2100)
which is produced often together with a related antibiotic,
suzukacillin by strains of Trichoderma viride. It can act as
an IONOPHORE [Book ref. 14, pp. 219224].
L-alanine biosynthesis See Appendix IV(b) and AMMONIA ASSIMILATION.
ala-P (AlaP) See ALAFOSFALIN.
alaphosphin Syn. ALAFOSFALIN.
Alaria See PHAEOPHYTA.
alarmone A low-MWt molecule, synthesis of which serves as
a trigger or signal for the redirection of cellular metabolism in
response to a particular type of stress; an example is ppGpp in
STRINGENT CONTROL (sense 1).
alastrim See SMALLPOX.
alazopeptin See DON.
albamycin Syn. NOVOBIOCIN.
Alberts stain A stain used to demonstrate METACHROMATIC
GRANULES. To prepare Alberts stain: TOLUIDINE BLUE (0.15 g)
and MALACHITE GREEN (0.2 g) are dissolved in 95% ethanol (2 ml)
and added to 1% acetic acid (100 ml); the whole is filtered after
standing for 24 h. A heat-fixed smear is stained with Alberts
stain (35 min), washed in tap water, and blotted dry; LUGOLS
IODINE is applied for 1 min and the smear washed and blotted
dry. Granules stain black, cytoplasm pale green.
albicidin An antibiotic, produced by Xanthomonas albilineans,
which inhibits DNA synthesis in Escherichia coli [JGM (1985)
131 10691075].
Alectoria
albofungin Syn. KANCHANOMYCIN.
albomycin See SIDEROMYCINS.
alborixin See MACROTETRALIDES.
Albugo A genus of obligately plant-parasitic fungi (order PERONOSPORALES) which are distinguished by their production of
basipetally formed chains of zoosporangia. A. candida (economically the most important species) is the causal agent of
white rust of crucifers (= crucifer white blister or white
blister disease). Within the tissues of the host plant, this fungus
forms a branching, aseptate, intercellular mycelium which produces rounded haustoria. The chains of zoosporangia develop
on short, club-shaped sporangiophores beneath the hosts epidermis, giving rise to smooth, white, blister-like lesions within
which the zoosporangia are compacted; subsequently, the epidermis ruptures, and the powdery mass of zoosporangia is dispersed
by wind and rain. During sexual reproduction, oogonia and
antheridia are produced within the host, and a fertilization tube
is formed between them; following fertilization and meiosis, the
oosphere gives rise to a thick-walled, warty oospore which later
germinates to form zoospores.
albumen The white of an egg. (cf. ALBUMINS.)
albumins A class of low-MWt proteins which are soluble in
dilute salt solutions and (unlike globulins) readily soluble in
water.
Alcaligenes A genus (incertae sedis) of catalase-positive, oxidase-positive, Gram-negative bacteria which occur e.g. in soil,
water, the alimentary tract in vertebrates, and in clinical specimens. Cells: non-pigmented rods (up to ca. 3.0 m in length),
coccobacilli, or cocci (ca. 0.51.0 m diam.), with 112 flagella per cell. Metabolism is respiratory (oxidative); all strains can
use O2 as terminal electron acceptor, and some can use nitrate
(anaerobic respiration). All strains can grow chemoorganotrophically on e.g. amino acids, acetate, fumarate, lactate, malate
or succinate carbohydrates being little used, although some
strains can use (and form acid from) glucose and/or xylose;
some (H2 -oxidizing) strains can grow chemolithotrophically.
The organisms usually grow well on e.g. peptone-containing
media and blood agar. Alkali is formed from the salts of certain
organic acids and from some amides. GC%: ca. 5670. Type
species: A. faecalis.
A. denitrificans. Most strains can reduce both nitrate and
nitrite to N2 . Strains of subsp. xylosoxydans are typically able
to use glucose and xylose, those of subsp. denitrificans are not.
The species includes strains previously named A. ruhlandii (H2 oxidizing organisms which have sheathed, peritrichous flagella),
and Achromobacter xylosoxidans.
A. faecalis. Most strains (including those previously named
A. odorans) can reduce nitrite but not nitrate. No chemolithotrophic strains have been reported.
A. odorans. See A. faecalis.
A. ruhlandii. See A. denitrificans.
Species incertae sedis [according to Book ref. 22, pp.
370373] include the peritrichously flagellated, aerobic,
H2 -oxidizing bacteria known as A. eutrophus, A. lactus
and A. paradoxus, and the non-fermentative, peritrichously
flagellated marine bacteria known as A. aestus, A. aquamarinus,
A. cupidus, A. pacificus and A. venustus (see DELEYA); these
organisms are considered not to belong to the genus Alcaligenes.
[Book ref. 22, pp. 361373.]
alcian blue A basic dye used e.g. for staining glycoproteins and
polysaccharides.
alcohol oxidase (alcohol:oxygen oxidoreductase; EC 1.1.3.13)
An enzyme (see ENZYMES) which oxidizes alcohols, giving the
Aleppo boil
e.g. on damp soil, on ice (ice algae see DIATOMS) and snow
(snow algae see RED SNOW), and on tree-trunks etc. Some
algae are photobionts in LICHENS or endosymbionts in various organisms (see e.g. ZOOCHLORELLAE and ZOOXANTHELLAE).
[Algal symbioses: Book ref. 129.] A few algae are parasitic
or pathogenic (see e.g. CHOREOCOLAX, HOLMSELLA, PROTOTHECA,
RED RUST). (See also ALGAL DISEASES.)
Certain algae have domestic and/or commercial or industrial
uses: see e.g. AGAR, ALGINATE, CARRAGEENAN, DIATOMACEOUS
EARTH, FUNORAN, FURCELLARAN, KELP, LAVER, NUNGHAM, SINGLECELL PROTEIN, YAKULT.
Algae are classified on the basis of their pigments, types
of storage carbohydrate, types and arrangements of flagella, CHLOROPLAST ultrastructure (including arrangement of
THYLAKOIDS) and CELL WALL composition. However, there is
currently no universally accepted taxonomic scheme which
encompasses all the algae; moreover alternative taxonomic
schemes coexist even within particular subgroups of algae: see
CHLOROMONADS, CHLOROPHYTA, CHRYSOPHYTES, CRYPTOPHYTES,
DIATOMS, DINOFLAGELLATES, EUGLENOID FLAGELLATES, PHAEOPHYTA, PRYMNESIOPHYCEAE, RHODOPHYTA, SILICOFLAGELLATES and
XANTHOPHYCEAE.
According to species, algae range from unicellular organisms
of a few micrometres to seaweeds of 50 metres or more in
length. (Unicellular organisms occur in most of the main groups
of algae cf. PHAEOPHYTA.) A CELL WALL is present in most algae
but is absent in a few unicellular algae (e.g. PORPHYRIDIUM).
The multicellular algae exhibit a great diversity of forms which
include branched and unbranched filaments or ribbons, sheets
of cells etc; in the thalli of some species there is considerable
differentiation e.g. in Laminaria spp the thallus includes
structures analogous to root, stem and leaf (holdfast, stipe and
blade, respectively) and a system of photosynthate-conducting
sieve tubes. (See also PNEUMATOCYST.) (Differentiation occurs
also e.g. in the unicellular alga ACETABULARIA.) Meristematic
tissue may occur in apical, intercalary and/or diffuse regions
depending e.g. on species. Some unicellular algae are motile
(see also MOTILITY). Colonial organization is exhibited by certain
microalgae (see e.g. COENOBIUM (sense 2) and PALMELLOID
PHASE).
Although normally photosynthetic, some algae (e.g. species
of CHLAMYDOMONAS, CHLORELLA and SCENEDESMUS) can grow
chemoorganotrophically, in the dark, on substrates such as
glucose or acetate; some algae (e.g. OCHROMONAS) can ingest
particulate food by phagocytosis.
Sexual reproduction (often oogamous) occurs in many algae,
and a number of algae exhibit an ALTERNATION OF GENERATIONS
which may be isomorphic (e.g. in Ectocarpus, Ulva) or heteromorphic (e.g. in Laminaria).
algal diseases ALGAE are subject to various diseases of microbial
aetiology, some of which are of economic importance in seaweeds cultivated for food etc. Thus, e.g., diseases of Laminaria
japonica (haidai) include frond twist disease caused by a
mycoplasma-like organism, and various rots caused by alginatedegrading bacteria; sporelings in culture may be killed by H2 S
produced e.g. by sulphate-reducing bacteria [Book ref. 130,
pp. 706708]. Porphyra spp are subject to red wasting disease (= red rot disease, Pythium red rot) caused by Pythium
spp [Experientia (1979) 35 443444], and to green spot disease caused by localized infection with species of Pseudomonas
or Vibrio. Various red algae may be attacked by Petersenia
spp: e.g. Petersenia palmariae infects Palmaria mollis [CJB
(1985) 63 404408, 409418]. Other microorganisms which
alkalophile
Alginates have a wide range of uses. Calcium alginate fibres
can be made by passing a solution of sodium alginate through
a spinneret immersed in a solution of calcium chloride acidified
with hydrochloric acid; calcium alginate is precipitated in the
form of continuous threads which may be processed (stabilized)
to form calcium alginate wool. This material (marketed as e.g.
Calgitex) is used as a COTTON WOOL substitute for making
SWABS or absorbent and absorbable surgical dressings. (Calcium
alginate swabs have been reported to be inhibitory when used
to prepare cultures of herpes simplex virus.) Calcium alginate
wool can be sterilized by autoclaving or by dry heat; it
can be dissolved e.g. in a 5% solution of sodium citrate or
in quarter-strength Ringers solution containing 1% sodium
hexametaphosphate. Thus, a swab carrying an inoculum can
be completely dissolved to release its entire complement of
microorganisms.
In industry, alginates are used e.g. as emulsifiers and thickeners in foods (alginates are easily digested), cosmetics, pharmaceuticals etc., and as supports for the IMMOBILIZATION of cells or
enzymes (for which purpose alginates rich in guluronic acid are
preferred as they form stronger gels).
alginate lyase (alginase) Any enzyme within the categories EC
4.2.2.3 and EC 4.2.2.11 which can degrade ALGINATE; such
enzymes have been isolated from many types of organism. [Alginate lyase (sources, characteristics, structurefunction analysis,
roles and applications): ARM (2000) 54 289340.]
alginic acid See ALGINATE.
algivorous Feeding on algae.
algology The study of ALGAE.
AlgU (sE ) See ALGINATE.
alicyclic hydrocarbons See HYDROCARBONS.
alimentary toxic aleukia A severe, usually lethal MYCOTOXICOSIS
caused by ingestion of mouldy grain contaminated with certain
TRICHOTHECENES usually T-2 toxin produced by Fusarium
tricinctum. Symptoms include extreme leucopenia and multiple
haemorrhages.
aliphatic hydrocarbons See HYDROCARBONS.
alkA gene See ADAPTIVE RESPONSE.
AlkalescensDispar group Non-motile strains of Escherichia
coli in which glucose is fermented anaerogenically and lactose
fermentation is delayed or absent.
alkaline peptone water See APW.
alkaline phosphatase See PHOSPHATASE.
alkaline phosphatase test See e.g. PHOSPHATASE TEST (for milk).
alkaliphile Syn. ALKALOPHILE.
alkalophile (alkaliphile) An organism which grows optimally
under alkaline conditions typically exhibiting one or more
growth optima within the pH range 811 and which
typically grows slowly, or not at all, at or below
pH 7. (cf. ACIDOPHILE.) Alkalophiles include a range of
bacteria e.g. certain Bacillus spp (including B. alcalophilus,
B. firmus and B. pasteurii ), Ectothiorhodospira abdelmalekii,
Exiguobacterium aurantiacum, species of Natronobacterium and
Natronococcus, and Thermomicrobium roseum and certain
fungi; the organisms occur e.g. in natural alkaline lakes and
in waters made alkaline by the effluents from certain industrial
processes (such as rayon manufacture). (Natural alkaline
environments are characterized by high concentrations of free
or complexed Na2 CO3 and usually by high concentrations of
NaCl.) A number of alkalophiles have an obligate requirement
for Na+ an ion important e.g. in SYMPORT processes; in at
least some flagellated alkalophiles flagellar rotation is driven
by SODIUM MOTIVE FORCE. However, in some species capable of
alkane metabolism
growth at neutral pH, Na+ is required only under non-alkaline
conditions. [Book ref. 192; the alkaline saline environment:
Book ref. 191, pp. 2554; genetic engineering of alkalophiles:
Book ref. 191, pp. 297315.]
alkane metabolism See HYDROCARBONS.
alkB gene See ADAPTIVE RESPONSE.
alkene metabolism See HYDROCARBONS.
alkylating agents Agents which react with nucleophilic groups
(e.g. amino, carboxyl, hydroxyl, phosphate, and/or sulphhydryl
groups) in e.g. proteins and nucleic acids, substituting them
with alkyl groups. (As commonly used, the term alkylating
agent is also applied to agents which substitute nucleophilic
groups with derivatives of alkyl groups: e.g. hydroxyethyl
groups in the case of ETHYLENE OXIDE.) Bifunctional alkylating
agents have two reactive groups and can cause cross-linking
between nucleophilic groups in proteins and/or nucleic acids (see
e.g. NITROGEN MUSTARDS and MITOMYCIN C). (See also SULPHUR
MUSTARDS.)
Depending e.g. on their reactivities, alkylating agents can
be effective antimicrobial agents and/or MUTAGENS. Some react
directly with cell components, others (e.g. alkyl-N-nitrosamines:
see N-NITROSO COMPOUNDS) require prior metabolic activation
(apparently to generate an alkyl carbonium cation). In general,
methylating agents are more reactive with DNA than are the
corresponding ethylating agents.
Alkylating agents form a range of products with DNA.
However, only some of the lesions are directly mutagenic: e.g.
O 6 -alkylguanine can pair with thymine during subsequent DNA
replication, resulting in GC-to-AT transitions, and alkylation
of the O-4 position of thymine can cause AT-to-GC transitions.
Most other lesions (e.g. N 7 -alkylguanine, N 3 -alkyladenine) are
not directly mutagenic, but they may be lethal unless repaired
by the cell (e.g. alkylation of the N-3 position of adenine blocks
replication forks); various DNA REPAIR systems can recognize and
repair alkylated bases (see e.g. ADAPTIVE RESPONSE).
The mutagenic effects of a given alkylating agent depend
largely on the nature of the lesions it produces. For example,
MNNG (q.v.), EMS (ethylmethane sulphonate) and MNU (Nmethyl-N-nitrosourea: see N-NITROSO COMPOUNDS) produce relatively more directly mutagenic lesions (particularly O 6 alkylguanine), while MMS (methylmethane sulphonate) produces higher proportions of e.g. N 7 -methylguanine and N 3 methyladenine but relatively little O 6 -methylguanine. However,
in organisms (such as Escherichia coli ) which have an inducible
error-prone repair system (see SOS SYSTEM), MMS can be mutagenic by causing lesions which induce this system; even in the
case of directly mutagenic agents such as MNNG, a proportion
of the mutations induced may be due to error-prone repair in
E. coli [JB (1985) 163 213220].
alkyldimethylbenzylammonium chloride See QUATERNARY AMMONIUM COMPOUNDS.
N-alkylnitrosoureas See N-NITROSO COMPOUNDS.
all-glass impinger (bubbler) An instrument used e.g. for sampling the airborne microflora. (See also AIR.) Essentially, it
consists of a vertical glass cylinder, containing a volume of liquid, and a longer, narrower glass tube fitted coaxially within
the cylinder and partly submerged in the liquid; when suction is
applied to the annular space, air is drawn in through the narrow
tube and bubbles up through the liquid during which process
particles are transferred from the air to the liquid.
allantoid Sausage-shaped; elongated and slightly curved with
rounded ends.
TEST.)
provokes a TYPE I REACTION. (See also PRAUSNITZKUSTNER
(2) A condition in which contact with a given allergen gives rise
to any manifestation of HYPERSENSITIVITY (see e.g. EXTRINSIC
ALLERGIC ALVEOLITIS). (3) Formerly, the condition of a PRIMED
individual.
allergy of infection An early name for DELAYED HYPERSENSITIVITY.
Allerton disease An African CATTLE DISEASE which involves
a mild febrile condition followed by the appearance of skin
nodules; it is caused by the bovine mammillitis virus and is
apparently similar or identical to pseudo-LUMPY SKIN DISEASE.
Allescheria boydii See PSEUDALLESCHERIA.
alloantigen Antigen from a genetically different individual of the
same species.
allochromasy Gradual, spontaneous chemical modification which
occurs in the solutions of certain dyes a single dye becoming
a mixture of dyes. (See e.g. polychrome METHYLENE BLUE and
NILE BLUE A.)
allochthonous Not indigenous to a given environment. (cf.
AUTOCHTHONOUS sense 1.)
alloenzyme See MULTILOCUS ENZYME ELECTROPHORESIS.
allogeneic Derived from a genetically different individual of the
same species. (cf. SYNGENEIC; XENOGENEIC.)
Allogromia See FORAMINIFERIDA.
Allogromiina See FORAMINIFERIDA.
allolactose b-D-Galactopyranosyl-(1 6)-D-glucopyranose: a
minor product of b-galactosidase action on LACTOSE; it is the
natural inducer of the LAC OPERON in Escherichia coli.
Allomonas A genus of bacteria (family VIBRIONACEAE) which
have been isolated from fresh water, sewage and faeces; GC%:
ca. 57. Type species: A. enterica [IJSB (1984) 34 150154].
Allomyces
A genus of fungi (order BLASTOCLADIALES) which
occur in moist soils, muds, and water. The thallus is a branched,
coenocytic mycelium which is attached to the substratum by
branching rhizoids; in at least some species the cell wall contains CHITIN. (See also CONCENTRIC BODIES.) Some species exhibit
an ALTERNATION OF GENERATIONS (q.v.). In e.g. A. macrogynus,
the sporothallus forms both thick-walled resistant sporangia
(meiosporangia) and thin-walled sporangia (mitosporangia);
the meiosporangia give rise to haploid zoospores (which
develop into gametothalli), while the mitosporangia form diploid
26
Alternaria
zoospores (which develop into new sporothalli). Terminal
branches of a gametothallus give rise to an orange-coloured
distal male gametangium and a colourless subterminal female
gametangium; the small male gametes fuse with the larger
female gametes, and the zygote germinates to form a sporothallus. (See also PHEROMONE.)
Species which do not exhibit sexual processes are sometimes
placed in the subgenus Brachyallomyces.
allopatric Existing in different environments or geographical
regions (cf. SYMPATRIC).
allophycocyanins See PHYCOBILIPROTEINS.
allotype Any one of a range of serologically distinguishable
variant forms of an Ig molecule produced as a consequence of
allelic variation in the Ig-specifying genes; a given allotype is
thus present only in those individuals who have the relevant
allele (cf. ISOTYPE). Different allotypes usually differ in amino
acid sequence in the constant region of their heavy or light
chains; sometimes the variable region is involved. Allotypes in
man include e.g. the Gm (G1m, G2m etc) allotypes of IgG.
allulose phosphate pathway Syn. RMP PATHWAY.
allylamines A group of synthetic ANTIFUNGAL AGENTS which
are highly active against dermatophytes and show somewhat
variable activity against yeasts (e.g. Candida spp), apparently
by inhibiting the enzyme squalene epoxidase; they include
naftifine and terbinafine. Terbinafine has in vitro activity against
Paracoccidioides brasiliensis [JCM (2002) 40 28282831].
Alnus root nodule See ACTINORRHIZA.
alopecia Loss of hair.
a (linking number) See DNA.
alpha chain (immunol.) See HEAVY CHAIN.
a-factor See MATING TYPE.
a-granules CYANOPHYCIN granules.
alpha interferon See INTERFERONS.
a operon See RIBOSOME (biogenesis).
a peptide (auto-a) A peptide (185 amino acids long) which
is cleaved from the N-terminus of the (lacZ-encoded) bgalactosidase of Escherichia coli e.g. during autoclaving. The a
peptide can restore some b-galactosidase activity to a population
of cells which, owing to a deletion mutation in lacZ, produce an
inactive enzyme lacking the N-terminal portion.
The lacZ sequence corresponding to the a peptide can be used
as a marker in a CLONING vector. During cloning, use is made
of a restriction endonuclease which cleaves at a site within this
sequence; thus any insertion of exogenous DNA will usually
result in loss of a peptide synthesis. The DNA is introduced
into suitable lacZ deletion mutants, and the cells are plated on
Xgal medium (see XGAL). Cells which receive the intact vector
form blue colonies (due to complementation between the a
peptide and the defective b-galactosidase), while those receiving
recombinant DNA usually form white colonies.
a1-a2 hypothesis See MATING TYPE.
Alphaherpesvirinae (herpes simplex virus group) A subfamily
of viruses of the HERPESVIRIDAE (q.v.). Alphaherpesviruses have
a short replication cycle (<24 hours); they spread rapidly in cell
cultures, causing mass lysis of susceptible cells.
The natural host range varies from narrow to wide, according
to virus. While, in cell cultures, latent infection with (nondefective) viruses does not occur readily, latent infection often
occurs in nerve ganglia within the living host.
The subfamily includes at least two genera: Simplexvirus
(human herpesvirus 1 group) and Poikilovirus (proposed name)
(suid herpesvirus 1 group) [Intervirol. (1986) 25 141143].
The type species of the genus Simplexvirus is human (alpha)
herpesvirus 1 (HERPES SIMPLEX virus type 1, HSV-1). The linear
alternaria rot
altro-heptulose Syn. SEDOHEPTULOSE.
Alu sequences In the human genome: a family of closely related,
dispersed sequences, each ca. 300 nt long, many of which
contain a common cleavage site for the restriction enzyme AluI;
Alu-like sequences occur in the genomes of other mammals and
of certain lower eukaryotes. (cf. REP SEQUENCE.)
AluI A RESTRICTION ENDONUCLEASE from Arthrobacter luteus;
AG/CT.
ALV AVIAN LEUKOSIS VIRUS.
alveolar membrane (protozool.) See PELLICLE (sense 3).
alveolitis Inflammation of the pulmonary alveoli. (cf. PNEUMONIA;
see also EXTRINSIC ALLERGIC ALVEOLITIS.)
alveolysin See THIOL-ACTIVATED CYTOLYSINS.
Alysiella
A genus of GLIDING BACTERIA (see CYTOPHAGALES);
A. filiformis occurs in the oral cavity in various vertebrates. The
organisms occur as flat filaments each composed of elongated
cells (23 m long) arranged side-by-side. Gliding occurs in a
direction perpendicular to the long axis of the cells i.e. along
the axis of the filament. Metabolism: chemoorganotrophic.
Alzheimers disease See CREUTZFELDTJAKOB DISEASE.
am mutant An amber mutant, i.e., a mutant with an amber
NONSENSE MUTATION.
amaas See SMALLPOX.
amanin See AMATOXINS.
Amanita A genus of fungi (AGARICALES, Amanitaceae) which
occur in deciduous and/or coniferous woodlands; some species
form mycorrhizal associations e.g. A. muscaria with birch
(Betula). According to species, the colour of the pileus may be
e.g. white, yellowish, red or brown. A. muscaria (the fly agaric)
forms a bright red pileus to which often adhere scattered white
scales (remnants of the universal veil). Some species are highly
poisonous; these include e.g. A. muscaria (see also MUSCARINE),
A. pantherina, A. phalloides (the death cap fungus), A. verna,
and A. virosa (the destroying angel). (See also AMATOXINS.)
Amanitaceae See AGARICALES.
a-amanitin An AMATOXIN which, at low concentrations, specifically inhibits eukaryotic RNA POLYMERASE II; RNA polymerase
III is inhibited at high concentrations.
amantadine (1-adamantanamine hydrochloride; 1-aminoadamantane hydrochloride) A polycyclic ANTIVIRAL AGENT (adamantane = tricyclodecane, C10 H16 ) which inhibits the replication of
certain viruses in tissue culture. It is used for the prophylaxis and
early treatment of INFLUENZA caused by type A influenzaviruses;
it can be administered orally or by aerosol.
At high concentrations, the action of amantadine is nonspecific: it raises the pH in endosomes and thus inhibits membrane fusion following endocytosis of a virus (see ENVELOPE).
At lower concentrations the drug selectively inhibits an early
stage in the infection of type A influenza viruses, the primary
target apparently being the M2 protein (see INFLUENZAVIRUS); the
activity of the drug results in failure of the pH-dependent fusion
of viral and vesicle membranes.
Rimantadine (a-methyl-1-adamantane methylamine hydrochloride) resembles amantadine in its spectrum of activity but
apparently causes fewer side-effects.
amanullin See AMATOXINS.
Amapari virus See ARENAVIRIDAE.
amastigote A form assumed by the cells of many species of
the TRYPANOSOMATIDAE (q.v.) during certain stages of their life
cycles. (See also LEISHMANDONOVAN BODIES.)
amatoxins Toxic cyclic peptides which occur in some species of
Amanita, e.g. A. phalloides, A. verna. In man, small quantities of
toxin (e.g. 5 mg) may be lethal; clinical effects are produced in
amino acids
ambruticin An antifungal antibiotic (a cyclopropylpolyenepyran acid) obtained from a strain of Polyangium cellulosum; it
shows in vitro activity against e.g. Candida spp, dermatophytes,
and other pathogenic fungi.
amdinocillin Syn. MECILLINAM.
ameba Syn. AMOEBA.
American foulbrood A BEE DISEASE which affects the larvae of
Apis mellifera usually after they have spun their cocoons; the
causal agent is Bacillus larvae. Infection occurs by ingestion of
food contaminated by spores of B. larvae. The spores germinate
in the gut, and the bacteria penetrate to the haemolymph and
multiply; the larvae die, turn brown, and putrefy. (cf. EUROPEAN
FOULBROOD.)
amerosporae See SACCARDOAN SYSTEM.
Ames test (Mutatest; Salmonella/microsome assay) A test for
detecting whether or not a particular agent is mutagenic (and
hence possibly carcinogenic) by determining its ability to
cause reversion to prototrophy in certain histidine-requiring
mutants of Salmonella typhimurium. Various tester strains of
S. typhimurium may be used, each having a different type of
MUTATION (frameshift, missense or nonsense) in the histidine
operon. Many of the strains used also contain mutations in uvrB
(preventing EXCISION REPAIR) and in rfa (causing LPS deficiency
and hence increased permeability to certain chemicals); most
contain the plasmid pKM101 which carries genes for error-prone
repair (see SOS SYSTEM) and which thus enhances the mutagenic
effects of DNA-damaging agents. Since certain chemicals are
mutagenic/carcinogenic only after metabolic activation, the test
commonly includes a preparation of microsomal enzymes from
a liver homogenate (9000 g supernatant, fraction S9) obtained
from rats pre-treated with a carcinogen (to induce the appropriate
enzymes).
The test may be carried out e.g. as a plate incorporation
test. A culture of a particular tester strain of S. typhimurium,
an S9 preparation, and the chemical under test are mixed with
soft agar containing a low concentration of histidine, and this is
poured onto a minimal agar plate; the whole is then incubated
at 37 C for 48 h in the dark. The low level of histidine permits
limited growth of the auxotrophic mutant cells, resulting in a
background of confluent light growth in the upper layer of agar
(top agar); any prototrophic revertants (whose growth is not
limited) can be seen as isolated colonies. In scoring revertants,
account must be taken of the (known) spontaneous reversion rate
for the strain used. (Absence of background growth implies that
the agent under test has general antibacterial activity, and any
colonies which develop are unlikely to be revertants.) The basic
test has been modified in various ways for particular purposes.
[Example of use with a carbamic acid derivative: AAC (2005)
49 11601168.]
(See also SOS CHROMOTEST.)
amicyanin A BLUE PROTEIN (MWt ca. 12000) present in certain
methylamine-utilizing bacteria (e.g. Pseudomonas AM1) see
METHYLOTROPHY.
Amies transport medium See TRANSPORT MEDIUM.
amikacin A semi-synthetic derivative of KANAMYCIN A which
contains an a-aminohydroxybutyric acid residue; it is more
active than kanamycin against e.g. Pseudomonas aeruginosa and
has been used against gentamicin-resistant strains.
aminacrine Syn. 9-AMINOACRIDINE.
amino acids For principal biosynthetic pathways see Appendix
IV; see also e.g. AROMATIC AMINO ACID BIOSYNTHESIS, GLUTAMIC
ACID, OPERON (attenuator control). For standard abbreviations for
amino acids see table.
9-aminoacridine
Aminoglycoside antibiotics are less effective under anaerobic
conditions and are ineffective against obligate anaerobes.
The aminoglycoside antibiotics are widely used therapeutically, sometimes in combination with other drugs. [Clinical roles
of aminoglycosides (symposium): Am. J. Med. (1985) 79 (1A)
176.] Side-effects (particularly with neomycin and streptomycin) include dose-dependent damage to the 8th cranial nerve
(associated with ototoxicity); kidney damage and hypersensitivity reactions are also possible.
Aminoglycoside antibiotics bind to the 30S ribosomal subunit
in bacteria some (e.g. streptomycin) bind at a single site while
others (e.g. gentamicin, kanamycin, neomycin) apparently bind
at multiple sites. They inhibit PROTEIN SYNTHESIS. For example,
low levels of streptomycin cause misreading of mRNA (i.e.
incorporation of incorrect amino acids) while higher levels
completely inhibit protein synthesis apparently by blocking
ribosomes specifically at the start of translation. There are other
sites of activity (e.g. the outer membrane in Gram-negative
bacteria), but the main effect of these antibiotics appears to result
from their influence on protein synthesis.
Resistance to aminoglycoside antibiotics can arise by several
distinct mechanisms: (i) mutation(s) in ribosomal proteins of the
30S subunit which can affect the binding of these antibiotics
(see e.g. STREPTOMYCIN); (ii) modification (inactivation) of
the antibiotics by plasmid-encoded or chromosome-encoded
bacterial enzymes which carry out O-phosphorylation, Nacetylation or O-adenylation; (iii) reduced uptake. [TIM (1998)
6 323327.]
Mutations giving one-step high-level resistance to aminoglycoside antibiotics are uncommon, but resistance to some
(e.g. spectinomycin, streptomycin) can occur in this way;
spectinomycin-resistant mutants do not show cross-resistance to
streptomycin, and streptomycin-resistant mutants do not show
cross-resistance to those antibiotics (e.g. kanamycin) which
appear to bind at multiple sites on the ribosome.
Aminoglycoside antibiotic-inactivating enzymes include
acetyltransferases (AACs), adenylyltransferases (AADs) and
phosphotransferases (APHs) [for nomenclature and sites of
action see: BMB (1984) 40 2835]. Some of these enzymes can
inactivate only a few aminoglycoside antibiotics while others
can inactivate many; some are found only in Gram-negative
species or in Gram-positive species, and some are found only in
e.g. Pseudomonas or Staphylococcus spp. Some of the enzymes
occur in a wide range of species. (See also e.g. Tn5 and Tn21 .)
Certain (mutant) bacteria exhibit drug-dependence in respect
of certain aminoglycoside antibiotics: see e.g. SPECTINOMYCIN
and STREPTOMYCIN.
6-aminopenicillanic acid (6-APA) A derivative of natural PENICILLINS (see b-LACTAM ANTIBIOTICS for structure): a precursor of
many semi-synthetic penicillins. 6-APA itself has little or no
antibacterial activity.
aminopeptidase See PROTEASES. (See also METHIONINE AMINOPEPTIDASE).
aminopterin See FOLIC ACID ANTAGONIST.
2-aminopurine See BASE ANALOGUES.
aminoquinolines A group of ANTIMALARIAL AGENTS that include
4-aminoquinolines (e.g. chloroquine, mefloquine, amodiaquine)
and 8-aminoquinolines (e.g. primaquine). The quinoline-type
antimalarials (including quinine) apparently kill the parasite
by preventing its detoxification of the ferriprotoporphyrin IX
by-product of haemoglobin metabolism (see HAEMOZOIN and
QUININE).
Chloroquine is an inexpensive synthetic drug which is used
orally for treating uncomplicated malaria. It has also been used
Three-letter
abbreviation
One-letter
abbreviation
Ala
Arg
Asn
Asp
Cys
Glu
Gln
Gly
His
Ile
Leu
Lys
Met
Phe
Pro
Ser
Thr
Trp
Tyr
Val
A
R
N
D
C
E
Q
G
H
I
L
K
M
F
P
S
T
W
Y
V
9-aminoacridine (aminacrine) A substituted acridine (see ACRIDINES) used e.g. as an ANTISEPTIC for the treatment of wounds,
and as a laser dye.
aminoacyl-tRNA synthetase See PROTEIN SYNTHESIS.
aminoadipic acid pathway (AAA pathway) A pathway for
lysine biosynthesis [see Appendix IV(e)] which occurs only in
certain lower fungi (Blastocladiales, Chytridiales, Mucorales),
ascomycetes (including e.g. Saccharomyces), basidiomycetes,
and euglenoid flagellates. [Review: CRM (1985) 12 131151.]
(cf. DIAMINOPIMELIC ACID PATHWAY.)
p-aminobenzoic acid (PABA; PAB) A component of FOLIC ACID.
PABA is synthesized from chorismate [see Appendix IV(f)].
Certain microorganisms e.g. Clostridium and Lactobacillus
spp require PABA as a growth factor. (See also PAS and
SULPHONAMIDES.)
7-aminocephalosporanic acid See CEPHALOSPORINS.
aminoglycoside antibiotics A class of broad-spectum ANTIBIOTICS; a typical aminoglycoside antibiotic contains an
aminosugar and either STREPTIDINE or (more commonly)
2-DEOXYSTREPTAMINE. [Book ref. 14, pp 418442, gives detailed
chemical structures.]
This group of antibiotics is generally taken to include
e.g. AMIKACIN, APRAMYCIN, butirosin, FRAMYCETIN, GENTAMICIN, hygromycin B, KANAMYCIN, KASUGAMYCIN, LIVIDOMYCIN,
NEAMINE, NEOMYCIN, netilmicin, PAROMOMYCIN, ribostamycin,
SISOMYCIN, SPECTINOMYCIN, STREPTOMYCIN and TOBRAMYCIN.
Many aminoglycoside antibiotics are bactericidal but some
(e.g. kasugamycin, spectinomycin) are bacteriostatic. Aminoglycoside antibiotics are active against both Gram-positive
and Gram-negative bacteria; at least some (e.g. gentamicin,
kanamycin, streptomycin) are inactive, or only weakly active,
against certain archaeans (methanogens [SAAM (1985) 6
125131]), while others (e.g. kasugamycin, neomycin, paromomycin, STREPTOMYCIN) are active against both prokaryotic and
eukaryotic microorganisms.
30
ammonification
mitotic divisions of each nucleus of the dikaryon in the ascus
mother cell. (cf. APOMIXIS.)
Ammodiscus See FORAMINIFERIDA.
Ammonia See FORAMINIFERIDA.
ammonia assimilation Ammonia can be used as the sole
source of nitrogen by many types of microorganism; it may
be obtained from an external source or produced intracellularly for example, by deamination reactions or by ASSIMILATORY NITRATE REDUCTION.
Ammonia can be taken up readily through the cytoplasmic
membrane; ammonium ions require a TRANSPORT SYSTEM [transport of ammonium ions in bacteria: FEMS Reviews (1985) 32
87100].
Within the cell, ammonia can be assimilated in different ways.
With high concentrations of ammonia, some bacteria (including Escherichia coli, Klebsiella spp) use ammonia for the
reductive amination of 2-oxoglutarate to L-glutamate in a reaction catalysed by NADPH-dependent glutamate dehydrogenase
(GDH; EC 1.4.1.2). L-Glutamate can act as an N-donor in
transamination reactions in which amino acids are synthesized from 2-oxoacids; E. coli synthesizes three low-specificity
transaminases: transaminase A (which preferentially catalyses
the synthesis of e.g. L-alanine and L-aspartate), B (aromatic
amino acids) and C (branched-chain amino acids).
With low concentrations of ammonia (e.g. <ca. 1 mM) many
bacteria and other organisms assimilate ammonia via a twostep reaction which is catalysed by (i) glutamine synthetase
(GS; EC 6.3.1.2) and (ii) glutamine:2-oxoglutarate aminotransferase (GOGAT; glutamate synthase; EC 1.4.1.13). In this
pathway, glutamate is initially aminated to glutamine in an ATPdependent, GS-catalysed reaction which consumes ammonia.
Then, in an NADPH-dependent, GOGAT-catalysed amination,
one molecule of glutamine and one of 2-oxoglutarate yield two
molecules of glutamate (see Appendix IV(a)). Many organisms
can use the initial (GS-catalysed) step for glutamine synthesis,
glutamine being used as a donor of amino groups in the
biosynthesis of e.g. purines, carbamoyl phosphate (a precursor
of pyrimidines), histidine and tryptophan.
In E. coli, it appears that the GDH-catalysed pathway is used
under energy-limiting conditions (the other pathway is ATPdependent). [Pathway choice in glutamate synthesis in E. coli :
JB (1998) 180 45714575.] Mutants of E. coli lacking both
pathways cannot use exogenous ammonia, but can grow on an
external source of glutamate.
In enterobacteria, the GDH and GS/GOGAT systems are
regulated at the level of transcription and (in the case of GS)
enzyme activity. High concentrations of ammonia repress the
synthesis of GS (and other nitrogen-regulated genes: see NTR
GENES) and induce the synthesis of GDH; this situation is
reversed when ammonia levels become limiting. GS activity
is controlled in response to ammonia levels, the enzyme being
inactivated by (reversible) adenylylation in the presence of high
levels of ammonia.
In e.g. Streptomyces venezuelae the anaerobic assimilation of
ammonia involves synthesis of alanine by the reductive amination of pyruvate via NADH-dependent alanine dehydrogenase
(EC 1.4.1.1) [CJM (1985) 31 629634].
In Streptomyces clavuligerus the GS/GOGAT pathway appears
to be the only one for ammonia assimilation [JGM (1986) 132
13051317].
ammoniacal silver nitrate See SILVER.
ammoniated mercury See MERCURY.
ammonification The formation of free ammonia (or NH4 + )
during the microbial breakdown of nitrogenous organic matter
Anabaena
(2) A copy of the specific nucleotide sequence which has
been amplified by a nucleic-acid-amplification technique such
as NASBA or PCR.
(3) A defective virus vector [e.g. PNAS (1985) 82 694698].
amplicon containment See PCR.
amplicon inactivation See PCR.
amplification (mol. biol.) See GENE AMPLIFICATION.
amplification pathway (immunol.) See COMPLEMENT FIXATION
(b).
amplified Mycobacterium tuberculosis direct test See TMA.
amplimer An alternative (though infrequently used) name for a
primer in a PCR reaction.
AmpliTaq Gold DNA polymerase See HOT-START PCR.
AmpliWax See HOT-START PCR.
ampoule Syn.VIAL.
AMPPD Trade name (Tropix, Bedford, MA, USA) of a 1,2dioxetane substrate which gives rise to CHEMILUMINESCENCE
when activated by the enzyme alkaline phosphatase.
amprenavir See ANTIRETROVIRAL AGENTS.
amprolium A coccidiostatic agent which is structurally similar
to thiamine.
ampulla (1) (protozool.) In certain ciliates (e.g. some hymenostomes): a channel, or the wider part of a channel, leading into
a contractile vacuole.
(2) (protozool.) In certain hypostome ciliates: an adhesive
organelle.
(3) (mycol.) The expanded, terminal region of some types of
conidiogenous cell (see CONIDIUM).
(4) (mycol.) The expanded, terminal region of some types of
conidiophore (see e.g. ASPERGILLUS).
Ampullariella
A genus of bacteria (order ACTINOMYCETALES,
wall type II) which occur e.g. in soil and freshwater habitats.
The organisms resemble Actinoplanes spp but differ e.g. in that
the rod-shaped zoospores are formed in parallel rows within the
cylindrical sporangium. Type species: A. regularis.
ampullate development See CONIDIUM.
ampulliform Flask-shaped.
Amsacta moorei EPV See ENTOMOPOXVIRINAE.
AMTDT See TMA.
AMU ATOMIC MASS UNIT.
amv See MYB.
AMV Avian myeloblastosis virus: see AVIAN ACUTE LEUKAEMIA
VIRUSES.
AMV reverse transcriptase See REVERSE TRANSCRIPTASE.
amygdaliform Shaped like an almond.
amygdalin A b-glycoside, present e.g. in bitter almonds, consisting of GENTIOBIOSE linked to mandelonitrile. On b-glucosidase
action (or acid hydrolysis), amygdalin yields hydrogen cyanide,
glucose and benzaldehyde.
amylases Enzymes which cleave glucosidic linkages in e.g.
STARCH or GLYCOGEN.
a-Amylases ((1 4)-a-D-glucan 4-glucanhydrolases, EC
3.2.1.1) are endoenzymes which have little action on terminal (1 4)-a-bonds or on bonds adjacent to (1 6)-a branch
points. They act on amylopectin and glycogen to form glucose, maltose and branched a-limit DEXTRINS, and on amylose
to form first maltose and maltotriose, then slowly on maltotriose to form maltose and glucose. a-Amylases are common
among microorganisms. They are obtained commercially mainly
from Bacillus spp (see also IMMOBILIZATION (sense 1)) and are
used e.g. for processing starch to form glucose syrups: insoluble starch granules are dispersed in water by heating, and the
starch is partially hydrolysed with thermostable a-amylases from
anabolism
be stopped or merely retarded. In some cases oxygen sensitivity
is believed to be due to the lack of enzymes such as CATALASE
and SUPEROXIDE DISMUTASE the cells thus lacking protection
against the toxic metabolites H2 O2 and O
. Another suggestion
2
is that an unacceptably high (positive or low negative) Eh may
lead to a high intracellular Eh which, in turn, may e.g. prevent
reduction in redox couple(s) which are normally freely reversible
within the growing organism, and/or cause irreversible oxidation
of vital components.
anaerobic (1) Refers to an environment in which oxygen is
absent. (cf. AEROBIC.) (2) Having the characteristic(s) of ANAEROBE(s).
anaerobic digestion The anaerobic breakdown of complex animal and/or plant materials to simple substances which include
a high proportion of gaseous and soluble products; it involves
a diverse range of organisms whose metabolic pathways are
closely interrelated, and occurs e.g. in benthic muds, in the
RUMEN and in certain types of SEWAGE TREATMENT plant (see
also TERMITEMICROBE ASSOCIATIONS).
Initially, polysaccharides, lipids and proteins are cleaved,
by extracellular enzymes, to (respectively) sugars, (usually)
fatty acids and glycerol, and amino acids; most polysaccharides including cellulose, pectins and starch are readily
cleaved, but LIGNIN is not readily degraded. The sugars and
other small molecules are fermented by various organisms (e.g.
species of Bacteroides, Clostridium, Selenomonas, Succinivibrio and Veillonella) to products which include acetate, butyrate,
ethanol, lactate, propionate and succinate together with carbon
dioxide and hydrogen. Propionate can be metabolized to acetate
and/or carbon dioxide by e.g. Desulfobulbus, Desulfonema and
Syntrophobacter. [Propionate and succinate degradation: JGM
(1985) 131 643650.]
Carbon dioxide and hydrogen are metabolized to acetate
by some bacteria (e.g. Acetobacterium woodii, Clostridium
aceticum see ACETOGENESIS) and to methane by certain
METHANOGENS. The scavenging of hydrogen by these organisms
creates conditions suitable for the growth of the so-called
obligate proton reducers or obligate hydrogenogens (see e.g.
SYNTROPHOMONAS) which metabolize ethanol, lactate (and
other products of the initial fermentation) to acetate and
hydrogen; for these organisms only protons can act as electron
acceptors, and the continual scavenging of the resulting
hydrogen is essential for their growth.
In some anaerobic ecosystems acetate is metabolized to
methane by e.g. Methanosarcina and/or oxidized to carbon
dioxide by SULPHATE-REDUCING BACTERIA (e.g. Desulfobacter
postgatei ) and sulphur-reducing species (e.g. Desulfuromonas
acetoxidans); the latter organisms form hydrogen sulphide as a
by-product. In the presence of high concentrations of sulphate,
the sulphate-reducing bacteria can inhibit METHANOGENESIS by
using both acetate and hydrogen. In the rumen, however, much
of the acetate is absorbed by the ruminant itself.
The process of anaerobic digestion results in an appreciable
reduction in the bulk of biodegradable solids a particularly
useful feature in SEWAGE TREATMENT. The conversion of organic
carbon to methane forms an important part of the CARBON CYCLE.
In sewage treatment (and in the treatment of other organic
wastes such as agricultural and food-industry effluents) anaerobic digestion can yield a rich, relatively odourless agricultural
fertilizer (rich in microbial biomass) and a useful fuel gas
(biogas, also called marsh gas, sewer gas, sludge gas) which
may contain 50% or more of methane; ca. 3070% of solids
may be converted to gases the actual proportion depending
anchor sequence
e.g. on the substrate(s), the initial percentage of solids and the
retention time.
anaerobic jar A container used for the incubation of materials
(e.g. inoculated media) in the absence of oxygen or, in general,
under gaseous conditions other than atmospheric. See e.g.
BREWER JAR, GASPAK, MCINTOSH AND FILDES ANAEROBIC JAR. (See
also HOLDINGFLUSH JAR PROCEDURE.)
anaerobic respiration RESPIRATION under anaerobic conditions,
the terminal electron acceptor being (according to species and/or
environmental conditions): fumarate, nitrate, nitrite, nitrous
oxide, elemental sulphur, sulphate etc. See e.g. DISSIMILATORY
SULPHATE REDUCTION, FUMARATE RESPIRATION, NITRATE RESPIRATION, SULPHUR RESPIRATION and DENITRIFICATION. (See also dissimilatory perchlorate reduction in the entry BIOREMEDIATION.)
anaerobiosis (1) The complete absence, or (loosely) the paucity,
of gaseous or dissolved elemental oxygen in a given place or
environment. In nature, such conditions occur e.g. in the bottom
muds of ponds and rivers and in the intestinal tracts of animals
(see e.g. RUMEN). (See also ANAEROBIC JAR and ROLL-TUBE
TECHNIQUE.) In aerobic habitats, anaerobic microenvironments
may be created by the consumption of locally available oxygen
e.g. by facultatively anaerobic organisms.
(2) Life in the absence of air.
Anaerobiospirillum A genus of Gram-negative bacteria (family
BACTEROIDACEAE). Cells: round-ended helical rods, 0.60.8
3.08.0 m, with bipolar tufts of flagella. Various sugars (e.g.
glucose, lactose, sucrose) are fermented, the major products of
glucose metabolism being succinate and acetate. GC%: ca. 44.
Type species: A. succiniciproducens, first isolated from dogs. [In
human bacteraemia: JCM (1998) 36 12091213. Ileocolitis in
cats: JCM (2004) 42 27522758.]
anaerogenic Refers to an organism which does not produce gas
from a given substrate.
Anaeroplasma A genus of obligately anaerobic, cell wall-less,
sterol-requiring bacteria (class MOLLICUTES) which occur e.g.
in the RUMEN. Cells: non-motile, coccoid to pleomorphic; plasmalogens are major components of polar lipids in the cytoplasmic membrane. Some strains are bacteriolytic, causing clearing
in agar media containing e.g. Escherichia coli. Carbohydrates
are fermented to e.g. acetic, formic and lactic acids (together
with propionic or succinic acid in some strains), ethanol and
CO2 . GC%: ca. 2934. Type species: A. abactoclasticum; other
species: A. bactoclasticum. [Nucleic acid relationships among
anaerobic mycoplasmas: JGM (1985) 131 12231227.]
Anaerovibrio A genus of Gram-negative bacteria (family BACTEROIDACEAE) which occur e.g. in the RUMEN. Cells: curved rods,
ca. 0.5 1.23.6 m; monotrichously (polarly) flagellated. Carbon sources include e.g. fructose, lactate and ribose; major fermentation products from these substrates include propionic and
acetic acids and CO2 . Fermentation of glycerol yields mainly
propionic acid. Lipolytic, producing clearing on linseed oil agar.
Type species: A. lipolytica.
ana-holomorph (mycol.) A fungus for which no sexual stage or
state has been identified. (See also DEUTEROMYCOTINA.)
anammox bacteria Bacteria able to oxidize ammonia to dinitrogen, anaerobically, using nitrite as electron acceptor [see e.g.
Nature (2003) 422 608611].
anamnestic response In persons or animals: a heightened
response to the second or subsequent administration of a particular antigen given some time after the initial administration;
thus, e.g., the concentration of specific antibody increases at a
rate much greater than that in response to the first dose of the
antigen. (See also BOOSTER.)
Ancistrocoma
animal viruses Viruses (see VIRUS) which can infect and replicate
in the cells of animals including mammals, birds, poikilothermic vertebrates and/or invertebrates. See table for general
features.
The host range for a given animal virus varies from very
narrow (e.g. in nature, rubella and variola viruses apparently
infect only man) to very wide (e.g. rabies virus can infect most
mammals, while ARBOVIRUSES can replicate in both invertebrates
and mammals). A virus may be transmitted from host to host
directly (by body contact), via aerosols (DROPLET INFECTION), via
food or water (see e.g. FOOD POISONING and POLYHEDRA), via a
VECTOR, etc; some viruses can be transmitted transovarially or
can cross the placenta and infect the fetus.
Probably, many virus infections in animals are asymptomatic,
but some can result in diseases ranging from mild and selflimiting (e.g. most cases of the COMMON COLD) to severe or
fatal (e.g. AIDS, RABIES, YELLOW FEVER). The virus may remain
more or less localized at the site of infection (e.g. in some
forms of HERPES SIMPLEX, and in PAPILLOMAS), or it may spread
systemically via the bloodstream, lymphatic system or nervous
system often replicating preferentially or only in a specific
tissue or organ. (See also TROPISM sense 2 and PERSISTENCE.)
Disease symptoms may be due e.g. to disturbances in host cell
structure and/or metabolism, host cell lysis, immune responses
in the host animal, etc. Animal viruses have been implicated in
certain cancers (see DNA TUMOUR VIRUS and ONCOVIRINAE) and
in other diseases of unknown causation e.g. atherosclerosis
(see MAREKS DISEASE), MULTIPLE SCLEROSIS, and even psychiatric
disorders (see BORNA DISEASE and RETROVIRIDAE).
Identification of animal viruses often cannot be based entirely
on clinical manifestations of infection: infection may be asymptomatic, different viruses can sometimes cause similar diseases
(see e.g. ENCEPHALITIS), and similar viruses may cause widely
differing diseases (see e.g. ENTEROVIRUS). Thus, identification
often depends on laboratory procedures: e.g., light MICROSCOPY
(for e.g. CYTOPATHIC EFFECT) or ELECTRON MICROSCOPY of clinical specimens; propagation of the virus in TISSUE CULTURE,
EMBRYONATED EGGS or living animals, followed by observation of any virus-induced effects; serological tests (e.g.
COMPLEMENT-FIXATION TEST, ELISA, HAEMADSORPTION-INHIBITION
TEST, HAEMAGGLUTINATION-INHIBITION TEST, IMMUNOFLUORESCENCE, IMMUNOSORBENT ELECTRON MICROSCOPY, NEUTRALIZATION
TEST, etc). TYPING (e.g. for epidemiological purposes) may
involve e.g. serological tests and/or nucleic acid HYBRIDIZATION
techniques. PCR-based examination may be used e.g. to identify
drug-resistance mutations [genotyping of HIV-1: Lancet (1999)
353 21952199].
In only a few cases can virus diseases in animals be
controlled by chemotherapy (see ANTIVIRAL AGENTS); in most
cases prevention is the only means of disease control. In humans,
this may involve e.g. vaccination, isolation of infected patients,
elimination of vectors, etc; SMALLPOX has been effectively
eradicated by such methods. Virus diseases of other animals may
be controlled by similar methods, and also e.g. by slaughter of
infected animals, quarantine of animals for transportation, etc.
Viruses which cause INSECT DISEASES are sometimes used in the
BIOLOGICAL CONTROL of insect pests.
(cf. PLANT VIRUSES.)
animalcules (Animaliculae) An archaic term for microscopic
organisms, particularly protozoa.
anisogamy The union of gametes which differ in form and/or
physiology. When the gametes differ in size, the larger
(macrogamete) is regarded as female, the smaller (microgamete)
as male. (See e.g. OOGAMY; cf. ISOGAMY.)
Angstr
om unit (A)
1010 m (= 101 nm).
anguibactin See SIDEROPHORES.
anguidine Diacetoxyscirpenol: see TRICHOTHECENES.
anicteric Without jaundice.
AN-IDENT See MICROMETHODS.
aniline dyes Dyes derived from aniline (aminobenzene, C6 H5
NH2 ), e.g., some TRIPHENYLMETHANE DYES.
36
anisotropic inhibitor
ANIMAL VIRUSES: basic characteristics
Genomea
dsDNA
monopartite, ccc, sc
monopartite (partially ds)
monopartite, linear
monopartite, strands covalently
joined at each end
monopartite (possibly sometimes
bipartite), linear
monopartite, linear, with 5 terminal protein
monopartite, ccc, sc
ssDNA
monopartite, linear; ve-sense, or
either ve- or +ve-sense
ccc
Nucleocapsid
symmetry
Virus familyb
(host typec in parentheses)
+
+
+
+/
helical
isometric
isometric
complex
Baculoviridae (I)
Hepadnaviridae (V)
Herpesviridae (V)
Poxviridae (V;I)
+/
isometric
Iridoviridae (I;V)
isometric
Adenoviridae (V)
isometric
Papovaviridae (V)
isometric
Parvoviridae (V;I)
Presence of
envelope
isometric
dsRNA (linear)
bipartite, with terminal protein
multipartite
isometric
isometric
Birnaviridae (V;I)
Reoviridae (V;I;P)
ssRNA (linear)
+ve-sense, monopartite
+ve-sense, monopartite
+ve-sense, diploid
+ve-sense, monopartite
+ve-sense, monopartite
+ve-sense, monopartite
+ve-sense, monopartite
+ve-sense, monopartite
+ve-sense, bipartite
ve-sense? monopartite
ve-sense, monopartite
ve-sense, monopartite
ve-sensee , bipartite
ve-sensee , tripartite
ve-sense, multipartite
+
+
+
+
+
+
+
+
+
+
+
helical
helical
isometric
isometric
isometric
isometric
isometric
isometric
isometric
helical
helical
helical
helical
helical
helical
Toroviridaed (V)
Coronaviridae (V)
Retroviridae (V;I?)
Togaviridae (V;I;P?)
Flaviviridae (V;I)
Caliciviridae (V)
Nudaurelia b virus group (I)
Picornaviridae (V;I)
Nodaviridae (I)
Filoviridaed (V)
Paramyxoviridae (V)
Rhabdoviridae (V;I;P)
Arenaviridae (V)
Bunyaviridae (V;I)
Orthomyxoviridae (V)
ssRNA (circular)
?-sense, monopartite
isometric
a
b
c
d
e
See entry VIRUS for generalized account. ccc = covalently closed circular; ds = double-stranded; sc = supercoiled; ss =
single-stranded.
See separate entries for details.
I = invertebrate; P = plant; V = vertebrate.
Proposed family.
Some segments are ambisense.
anisotropic medium
to sites in Complexes I, III and IV of the mitochondrial ELECTRON
and to the F0 moiety of the PROTON ATPASE.
anisotropic medium (optics) See BIREFRINGENCE.
Ankistrodesmus A genus of unicellular, non-motile green algae
(division CHLOROPHYTA); the cells are generally long and thin
and may be straight, curved, helical etc, sometimes occurring in
bundles. (See also TBTO.)
anlage (pl. anlagen) (ciliate protozool.) Syn. INITIAL(S).
annealing (of primers) See PCR.
annelate ascus An ASCUS whose wall has a small, annular, apical
thickening that is often amyloid or light-refractive; at maturity,
the ascospores are released via a pore in the centre of the
thickening.
annellations See CONIDIUM.
annellide See CONIDIUM.
annellidic development See CONIDIUM.
annulus (microbiol.) Any of various structures which are ringshaped (either actually or in cross-section). Examples include
e.g. the outermost layer (= sheath) of the contractile stalk in
some peritrich ciliates, the PERISEPTAL ANNULUS, and the annular
remnant of the PARTIAL VEIL.
Anodonta See ZOOCHLORELLAE.
Anomoeoneis See DIATOMS.
anonymous mycobacteria Syn. ATYPICAL MYCOBACTERIA.
Anopheles A genus of mosquitoes (order Diptera, family Culicidae); Anopheles spp are vectors of MALARIA.
anopheline Refers to mosquitoes of the genus Anopheles.
Anoplophrya See ASTOMATIDA.
anorthoploid Syn. ANEUPLOID.
anoxia A deficiency or lack of oxygen. (Hence adj. anoxic.)
anoxygenic Not producing oxygen.
anoxygenic photosynthesis See PHOTOSYNTHESIS.
Anoxyphotobacteria A proposed class of anoxygenic photosynthetic prokaryotes (division GRACILICUTES): see RHODOSPIRILLALES.
ansamycins A group of structurally related ANTIBIOTICS consisting of a macrocyclic ring which comprises an aromatic moiety
spanned by an aliphatic bridge. Ansamycins (which include e.g.
rifamycins, streptovaricins and tolypomycins) are produced by
actinomycetes and appear to share a common mode of antibacterial action (see RIFAMYCINS); at high concentrations they also
show activity against certain viruses in cell cultures.
anserid herpesvirus 1 See DUCK VIRUS ENTERITIS.
antagonism The inhibition of one entity by another of similar
kind. Examples: one antibiotic may reduce or abolish the effects
of another (e.g. a bacteriostatic drug will counteract the effects
of a drug which acts only on growing cells); acid-producing
organisms may inhibit or kill acid-intolerant organisms sharing
the same environment. (cf. SYNERGISM.)
antapical organelle In the bacterium Thiovulum majus: the
presumed source of a thin (adhesive?) thread or stalk which
projects from the surface of the organism.
antenna (in PHOTOSYNTHESIS) See LIGHT-HARVESTING COMPLEX.
anterior station (parasitol.) The anterior part of the alimentary
canal and/or the salivary glands of an arthropod vector; infective
forms of parasites in the anterior station can be transmitted to
the vertebrate host by the bite of the vector. (cf. INOCULATIVE
INFECTION.)
antheraxanthin See CAROTENOIDS.
antheridiol See PHEROMONE.
antheridium A male gametangium.
anthracnose Any of various plant diseases particularly those
caused by fungi of the MELANCONIALES in which discrete, darkcoloured, necrotic lesions develop on the leaves and/or fruits.
TRANSPORT CHAIN
38
antibiotic
the sum of their individual effects; cotrimoxazole is an example
of a synergistic combination of antibiotics (trimethoprim + sulphamethoxazole) two drugs which block different reactions in
the same pathway.
Antagonism is the converse of synergism. For example,
antibiotics which inhibit growth will antagonize other antibiotics
(e.g. penicillins) which are active only on growing cells. In
another form of antagonism, the presence of certain types of
antibiotic will promote the synthesis of inducible enzymes that
inactivate other antibiotics; thus, for example, certain b-lactam
antibiotics (such as imipenem or cefoxitin) can induce the
synthesis of enzymes called b-lactamases which inactivate other
b-lactam antibiotics. (For this reason, those b-lactam antibiotics
which are strong inducers of b-lactamases are not used in
combination with other b-lactam antibiotics.)
The antimicrobial activity of an antibiotic in the human (or
animal) body does not necessarily correspond to its activity
in laboratory tests. For example, under in vivo conditions an
antibiotic may bind to plasma proteins so that only a fraction
of the administered dose is available for antimicrobial activity.
Moreover, some antibiotics are administered in an inactive form
that depends on in vivo metabolism for the development of its
activity (see e.g. p-N-succinylsulphatriazole in SULPHONAMIDES).
The ability of certain antibiotics (e.g. fluoroquinolones,
rifampicin) to remain in an active state within phagocytes is
an important feature because some bacterial pathogens can survive, or even grow, following uptake by phagocytic cells [RMM
(1995) 6 228235].
Antibiotic action. To be effective an antibiotic must (at least)
enter the cell envelope; commonly, antibiotics must pass through
the cell envelope in order to reach their target sites. Entry into a
cell often occurs via an energy-dependent transport system (see
e.g. entries CYCLOSERINE, POLYOXINS, TETRACYCLINES, WARHEAD
DELIVERY).
Within the pathogen, a given antibiotic acts at specific target
site(s). Depending on antibiotic, the target site may be e.g.: (i)
enzymes that catalyse the synthesis of a structural polymer in the
cell envelope; (ii) the cytoplasmic membrane (certain antibiotics
cause leakiness incompatible with cell viability); (iii) enzymes
required for the synthesis or supercoiling of nucleic acids; (iv)
the ribosome (some antibiotics can inhibit protein synthesis by
binding to specific sites on the ribosome); (v) enzymes required
for biosynthesis of an essential coenzyme for example, dihydrofolate reductase (required for the synthesis of tetrahydrofolate) is inhibited by trimethoprim.
Antibiotics of the same group have similar or identical target
sites, and they all affect cells in the same way. However, antibiotics from different groups may have a similar target site; thus,
for example, the target site of oxazolidinones appears to overlap
the binding sites of both lincomycin and chloramphenicol [JB
(2000) 182 53255331].
Some target sites are found in only certain categories of
microorganism; for example, the cell wall polymer peptidoglycan occurs only in bacteria so that antibiotics directed specifically against this target are unlikely to be of use against (e.g.)
fungi. Clearly, no antibiotic is effective against all pathogens,
and in many cases the activity of a given antibiotic is limited
to a particular subset of organisms; in the context of bacterial pathogens, a broad-spectrum antibiotic is one which can be
effective against a wide range of species, including both Grampositive and Gram-negative bacteria.
Some examples of antibiotics (in various target regions) are
listed below; see individual entries for mode of action etc.
antibiotic
Bacterial cell wall (peptidoglycan).
CYCLOSERINE;
b-LACTAM
DEPSIPEPTIDE ANTIBIOTICS;
ACTINOMYCIN D; ANTHRACYCLINE
40
antibody
essential for the synthesis of lipid A (an integral part of the
outer membrane in Gram-negative bacteria) (see ENDOTOXIC
SHOCK). New approaches to antibiotics may also involve agents
such as CcdB (see F PLASMID) and certain bacteriocins. By
contrast, peptide deformylase (PDF), which cleaves the Nterminal formyl group from nascent bacterial polypeptides (see
PROTEIN SYNTHESIS), seems less than optimal as a candidate
drug target; certain derivatives of hydroxamic acid are potent
inhibitors of PDF, but resistance to these agents develops readily,
and the drugs appear to be only bacteriostatic [AAC (2001) 45
10581064].
The ongoing problem of antibiotic-resistant pathogens has
prompted consideration of other anti-infection modalities, including bacteriophage therapy [AAC (2001) 45 649659].
Antibiotics for chemotherapy: factors affecting the choice.
Antibiotics may be wasted if they are used without due regard
to specificity and pharmacology; moreover, use of inappropriate
drugs may forfeit the chance of helping the patient and may
also exacerbate unnecessarily the general problem of antibiotic
resistance. The kind of factors which affect the choice of antibiotic include:
Effectiveness against relevant pathogens. In ideal circumstances the pathogens identity and its sensitivity to antibiotics
are known prior to treatment. However, in certain diseases
(e.g. meningitis) therapy is often begun before the aetiology
has been confirmed. When this happens the choice of antibiotic is based on the probable pathogen; probability reflects
factors such as (local) prevalence of particular species/strains
of pathogen, reported problems of resistance in the pathogen,
and the patients age/general condition. [Example: management of bacterial meningitis (paediatric patients): RMM
(1997) 8 171178.]
Prevalence of antibiotic-resistant strains in the locality. Many
pathogens are now resistant to antibiotic(s) to which they
were once invariably sensitive; moreover, some pathogens are
resistant to a range of drugs so that, in some cases, therapeutic
options are extremely limited.
Antagonism towards other antibiotics or even towards other
therapeutic agents; for example, rifampicin can potentiate
certain mammalian enzymes and, as a consequence, may
interfere with oral contraception.
Possible side-effects (e.g. penicillin allergy).
In pregnant patients: possible teratogenicity.
Pharmacokinetics. The physicochemical nature of a drug
determines its ability to reach particular sites when administered via a given route. For example, if certain drugs are
injected intravenously they do not reach the cerebrospinal
fluid (CSF) because they cannot pass the bloodbrain barrier; other types of drug can, and some can do so only if the
permeability of this barrier has been increased e.g. as a result
of inflammation.
(See also ANTIFUNGAL AGENTS, ANTIPROTOZOAL AGENTS, ANTIand DISINFECTANTS.)
antibiotic-associated colitis See COLITIS.
antibody (ab) Any IMMUNOGLOBULIN molecule produced in direct
response to an ANTIGEN (or to an autocoupling HAPTEN) and
which can combine specifically, non-covalently, and reversibly
with the antigen which elicited its formation (see also ANTIBODY
FORMATION); specificity is not necessarily absolute: see CROSSREACTING ANTIBODY. (A MYELOMA can produce Ig with antibody
function in the absence of antigenic stimulation. See also PASSIVE IMMUNITY.) The term antibody is also used to refer to a
SEPTICS
41
antibody absorption
which promotes activation and clonal proliferation of the T
cell and induces it to release cytokines, including INTERLEUKIN-4.
However, once activated, T cells produce the cell-surface antigen
CTLA-4 (= CD152), a molecule (similar to CD28) to which B7.1
and B7.2 can bind; interaction between B7.1/B7.2 and CTLA-4
may initiate a signal which terminates synthesis of IL-2 in the
T cell. (Note that, while IL-2 is not a characteristic product of
the Th2 subset of T cells, transient synthesis of this cytokine at
an early stage would appear to be necessary as it seems to be
an essential growth factor for T cells.)
Yet another paired interaction between the B and T cells
involves CD40 (q.v.).
The mutual (physical) co-operation between the B cell and T
cell (described above) is referred to as cognate help or linked
recognition.
The activated, proliferating B cells form an expanded clone.
Some of the cells of this clone become antibody-secreting
PLASMA CELLS. Others become MEMORY CELLS; these cells do not
secrete antibody but retain the potential to do so, rapidly, if subsequently challenged with the same antigen (giving a heightened
secondary response). (See also ANAMNESTIC RESPONSE.)
Initially, antibodies secreted by plasma cells are of the IgM
class. Subsequently, plasma cells form antibodies of another
class generally IgG but of the same specificity; such class
switching (= isotype switching) is promoted by several stimuli including the binding of B cell antigen CD40 to the corresponding T cell ligand, and the activity of the T-cell-derived
cytokine INTERLEUKIN-4.
Class switching occurs in so-called germinal centres within
lymph nodes and spleen. Such sites are also involved in a process
known as affinity maturation; in this process, mutant cells
among the (proliferating) antigen-stimulated B cells are selected
for high-affinity binding to the specific antigen selective
pressure presumably being a falling concentration of the given
antigen. Within the B cells a process known as somatic
hypermutation gives rise to mutations that are concentrated in
the V regions of antibody genes; as a consequence, different
B cells produce antibodies with different levels of affinity
for the given antigen those producing antibody with the
highest affinity being selected. [Hypermutation in antibody
genes: PTRSLB (2001) 356 1125.] (See also RNA EDITING.)
In the response to an antigen not previously encountered (a
primary response) the numbers of specifically reactive B cells
(prior to clonal expansion) are likely to be low. Under these
conditions it may be that the presentation of antigen to T cells
is carried out not by B cells but by other, more numerous,
APCs such as macrophages or dendritic cells. In this scenario,
interaction between APC and T cell activates the T cell which
then secretes various cytokines; these cytokines may induce
differentiation, proliferation and antibody secretion in B cells
that have bound the specific antigen and which are close to
(though not necessarily in contact with) the activated T cells
[Book ref. 227, pp 207208].
When produced in response to invasion by pathogens (or their
products e.g. toxins), antibodies commonly have a protective
role (see e.g. ADCC and OPSONIZATION). However, under certain
conditions, antibodies can promote damage to the hosts tissues
(see IMMEDIATE HYPERSENSITIVITY).
anticapsin See BACILYSIN.
anticlinal Perpendicular to a given surface. (cf. PERICLINAL.)
anticoagulant Any agent which inhibits the coagulation (clotting) of blood e.g. EDTA, HEPARIN, sodium citrate, sodium
oxalate. SPS is used in BLOOD CULTURE.
antigenic formula
The surface of a microorganism typically consists of repeating patterns of antigens, and the classification of some groups
of microorganisms is based on differences between the antigens
of different strains (see e.g. KAUFFMANNWHITE CLASSIFICATION).
(See also e.g. ALLERGEN; ANTIBODY; ANTIGENIC VARIATION; IDIOTYPE; IMMUNIZATION; THYMUS-DEPENDENT ANTIGENS.)
antigen-binding cell (ABC) (1) Any cell which can bind only
a specific antigen. (2) Any cell (including e.g. macrophages)
which can bind various antigens.
antigen deletion In a microorganism: the loss of particular
antigenic determinant(s) due e.g. to a mutation or to the loss
of a plasmid. (cf. ANTIGEN GAIN.)
antigen excess The presence of a high antigen-to-antibody ratio.
Under conditions of gross antigen excess precipitation does
not occur since, according to the LATTICE HYPOTHESIS, all the
combining sites of antibodies are bound to otherwise unattached
antigens leaving no combining sites free to form cross-links
and hence larger (insoluble) complexes. (See also TYPE III
REACTION.)
antigen gain In a microorganism: the formation of new antigenic
determinant(s). Antigen gain may be due e.g. to a MUTATION,
to the acquisition of a PLASMID, or to BACTERIOPHAGE CONVERSION; thus, e.g., the sex factor in a conjugative plasmid specifies
certain donor-specific antigens, while certain cell-surface antigens in Salmonella strains are present only when the cells are
lysogenized by a particular phage. (cf. ANTIGEN DELETION.)
antigen-presenting cell (APC) Any of a range of cells which
bind antigen and present it to an antigen-specific T cell. APCs,
which bear MHC class II cell-surface molecules (see HISTOCOMPATIBILITY RESTRICTION), include B LYMPHOCYTES, macrophages,
dendritic cells, Langerhans cells and Kupffer cells.
antigen-specific T helper cell A T LYMPHOCYTE which is specific
for, i.e. activated by, a given, specific antigen; such a T cell may
give COGNATE HELP to a B cell which has bound the same antigen
(see ANTIBODY FORMATION). (See also CARRIER-SPECIFIC T HELPER
CELL.)
antigenic (1) Syn. immunogenic (see IMMUNOGENICITY). (2) Of
or pertaining to an ANTIGEN or antigens.
antigenic competition Inhibition of the immune response to
a given antigen or DETERMINANT due to exposure to another
(different) antigen or determinant; antigenic competition has
been regarded as a form of natural immunosuppression.
In intermolecular competition, suppression of the response
to a given antigen may occur as the result of the previous
administration of the other antigen (sequential competition) or
of the simultaneous administration of the other antigen. By
carefully adjusting (balancing) the relative amounts of the
antigens, antigenic competition may be reduced or abolished;
this is important e.g. in the preparation of MIXED VACCINES.
In intramolecular competition the response to a given determinant is inhibited by the presence of another determinant on the
same macromolecule. For example, with IgG as antigen, good
titres of anti-Fc may be produced but relatively few anti-Fab antibodies are formed fewer than would be formed against isolated
Fab fragments (i.e., relative to Fab, Fc is immunodominant).
antigenic determinant See DETERMINANT.
antigenic drift (immunological drift) In a given species, strain
or type of microorganism: minor changes in antigenic specificity
which occur over an extended period of time (e.g. years) see
e.g. INFLUENZAVIRUS. (cf. ANTIGENIC SHIFT; ANTIGENIC VARIATION.)
antigenic formula Any symbolic notation which indicates the
antigenic nature of an organism see e.g. KAUFFMANNWHITE
CLASSIFICATION.
antigenic shift
antimalarial agents (antimalarials) Drugs which are effective
in the chemotherapy and/or chemoprophylaxis of MALARIA. Most
of these drugs are effective against only one stage of the malaria
parasite e.g. chloroquine, mefloquine, quinine and QINGHAOSU
are SCHIZONTICIDES. Primaquine and WR238605 are both active
against hypnozoites; primaquine is also active against tissue
schizonts (i.e. schizonts within liver cells), and WR238605 is
also active against gametocytes.
(See AMINOQUINOLINES, QINGHAOSU, QUININE, PYRIMETHAMINE
and MALARIA for details of antimalarials.)
Combinations of antimalarials are often used for treatment;
this helps e.g. to limit the emergence of resistant strains of the
parasite.
antimetabolite A substance which competitively inhibits the utilization, by an organism, of an exogenous substrate or endogenous metabolite. (See e.g. SULPHONAMIDES.)
antimony (as an antimicrobial agent) Antimony is a HEAVY METAL whose compounds have long been used as therapeutic
agents though their toxic effects were often greater than the
benefits they bestowed. Antimonials have found use in the treatment of certain diseases of protozoal aetiology, e.g. leishmaniasis, and other diseases, e.g. schistosomiasis. It is believed
that trivalent antimony is necessary for antimicrobial activity,
and that pentavalent compounds owe their activity to in vivo
conversion to the trivalent state. Antimonials have been shown
to combine with essential sulphhydryl groups in trypanosomal enzymes involved in glucose metabolism; such inhibition
may be reversed by thiol compounds, e.g. cysteine. Trivalent
antimonials include e.g. potassium antimonyl tartrate (tartar
emetic; 2[K(SbO).C4 H4 O6 ].H2 O) and stibophen (sodium antimony bis[pyrocatechol-3,5-disulphonate]). Pentavalent antimonials include e.g. stibanilic acid (p-aminobenzenestibonic acid)
and its sodium salt (stibamine), both of which are constituents of a
number of widely-used drugs e.g. ethyl stibamine (neostibosan)
which is used for the treatment of espundia and kala-azar.
antimutator gene See MUTATOR GENE.
antimycin A An antibiotic which acts as a RESPIRATORY INHIBITOR
in Complex III of the mitochondrial ELECTRON TRANSPORT CHAIN,
apparently blocking electron flow between b-type cytochromes
and cyt c1 ; antimycin A and HOQNO appear to act at a common
site which may be associated with the b-type cytochromes.
antimycotic See ANTIFUNGAL AGENTS (a).
antioxidant (food sci.) A substance added to certain foods to
inhibit oxidation of the lipids in those foods thus enhancing
stability and prolonging shelf-life. (See also OXIDATIVE RANCIDITY.) Antioxidants currently used include e.g. ascorbic acid,
butylated hydroxyanisole, butylated hydroxytoluene, carotene,
propylgallate and tertiary butylhydroquinone. Some antioxidants
have antimicrobial properties [CRM (1985) 12 153183].
antiparallel (of DNA strands) See DNA.
antiplectic metachrony See METACHRONAL WAVES.
antiport (counter transport, exchange diffusion) The transmembrane transport of a solute (e.g. a given ion) coupled, directly, to
the transmembrane transport of a different solute in the opposite
direction. (cf. SYMPORT, UNIPORT; see also ION TRANSPORT.)
antiprotozoal agents Chemical agents which kill or inhibit protozoa; they include e.g. AMINOQUINOLINES; antimonials (see
ANTIMONY); arsenicals (see ARSENIC); certain DIAMIDINES; DILOX-
antigenic shift In a given species, strain or type of microorganism: major change(s) in antigenic specificity which apparently occur abruptly. For example, antigenic shifts in strains of
INFLUENZAVIRUS have been reported to coincide with pandemics
of influenza. (cf. ANTIGENIC DRIFT; ANTIGENIC VARIATION.)
antigenic variation Successive changes which occur in the
surface antigens of certain microorganisms; in some cases, each
alternative antigen results from the expression of a specific allele
(see PHASE VARIATION), but in other cases (e.g. the fimbriae of
Neisseria see below), successive new antigens are created by
repeated recombinational events.
Antigenic variation may help a pathogen to evade the hosts
immune defence system; thus, e.g. new antigenic forms of
the pathogen which arise in the host may not be susceptible
to OPSONIZATION by those antibodies which have developed in
response to the previous antigenic forms.
Antigenic variation occurs e.g. in Borrelia (see RELAPSING
FEVER), INFLUENZAVIRUS, visna virus, Leishmania, Plasmodium
and Trypanosoma spp (see VSG).
The major structural subunit in the fimbriae of Neisseria gonorrhoeae (which are type IV FIMBRIAE) is encoded by the chromosomal gene pilE. The chromosome also contains copies of a
gene, pilS, with which pilE can undergo repeated RECOMBINATION; moreover, recombination can also occur between pilE and
any homologous DNA acquired through transformation. Recombinational events continually create new versions of the subunit
gene, so that the fimbriae of this organism can be synthesized
from any one of a very large number of variant forms of the
subunit, giving rise to extensive antigenic variation [Mol. Microbiol. (1996) 21 433440]. These fimbriae are also subject to
phase variation (on/off switching). (The Opa adhesins of Neisseria undergo phase variation by DNA re-arrangements that alter
reading frames in opa genes [TIM (1998) 6 489495].)
[An update of antigenic variation in African trypanosomes:
TIP (2001) 17 338343.]
antigenicity The capacity to function as an ANTIGEN. (cf. IMMUNOGENICITY.)
antiglobulin (Coombs reagent) Antibody homologous to the
antigenic determinants of serum globulins, particularly IMMUNOGLOBULINS; antiglobulinIg combination can occur without
involvement of the specific COMBINING SITES of the Ig molecule.
antiglobulin consumption test (serol.) Any CONSUMPTION TEST
in which the presence of cell- or particle-bound Ig is detected
by the consumption of added ANTIGLOBULIN. For example, the
in vitro combination of autoantibodies with homologous cellsurface antigens can be detected by washing the cells free of
uncombined antibody and incubating them with antiglobulin;
if autoantibodyantigen combination has occurred, antiglobulin
will be consumed and may cause agglutination by the formation
of cellautoantibodyantiglobulin complexes. The amount of
antiglobulin consumed can be determined e.g. by titrating the
unconsumed antiglobulin against Ig-coated erythrocytes.
antiglobulin test (serol.) Any test in which the presence of
Ig (including BLOCKING ANTIBODIES, sense 1) is detected by
exploiting the ability of ANTIGLOBULIN to agglutinate Ig-bound
antigens.
anti-idiotype Antiserum to the variable-region domains of an
Ig molecule (cf. IDIOTYPE); it contains antibodies homologous
to each of the individual determinants (IDIOTOPES), though the
different types of antibody may differ quantitatively and in their
AFFINITY for their respective determinants.
antilymphocyte serum (ALS) Antiserum to the cell-surface
antigens of LYMPHOCYTES; it is used e.g. for IMMUNOSUPPRESSION.
Antilymphocyte globulin (ALG) is the globulin fraction of ALS.
Aphanizomenon
4 C for several hours (or 37 C for ca. 15 minutes) to allow
antibodystreptolysin O combination a fixed volume of RBC
suspension is added to each dilution, and incubation carried out
at 37 C for 3045 minutes. Complete absence of haemolysis in
a given tube indicates that streptolysin O in that tube has been
fully neutralized by antibodies. The ASOT titre (often expressed
in TODD UNITS) is given by the highest dilution of serum which
completely inhibits haemolysis. ASOT can also be carried out
as a LATEX PARTICLE TEST using streptolysin O-coated particles.
antitermination A process in which, during TRANSCRIPTION, the
RNA polymerase fails to recognize a transcription termination
signal and therefore continues transcription beyond the terminator. Antitermination may involve various mechanisms and can
serve as a means for the regulation of gene expression (see e.g.
BACTERIOPHAGE LAMBDA (gpN ) and OPERON (attenuator control))
and for the prevention of erroneous transcription termination (see
e.g. RRNA).
antitoxin (1) An antibody to a toxin. (2) An antiserum which
contains antibodies to one or more particular toxins.
antiviral agents Agents which inhibit the replication of viruses
in cells, tissues or organisms either directly (e.g. by inhibiting
a specific viral enzyme) or by inducing the synthesis of
INTERFERON. (See also TILORONE.)
Owing to poor selective toxicity and/or the ready emergence
of resistant strains of virus, relatively few compounds which
exhibit antiviral activity in cell cultures are suitable for clinical
use, and many of these are limited to topical treatment of
localized infections.
ANTIRETROVIRAL AGENTS (q.v.) are antiviral agents used e.g. in
chemotherapy against AIDS.
Examples of antiviral agents include: ACYCLOVIR, AMANTADINE, ANSAMYCINS, ARABINOSYL NUCLEOSIDES, ARILDONE, BROMOVINYLDEOXYURIDINE, CYCLARIDINE, DHBG, DHPA, DHPG,
DIDEMNINS, ENVIROXIME, EPIPOLYTHIAPIPERAZINEDIONES, FAMCICLOVIR, GANCICLOVIR, IDOXURIDINE, LAMIVUDINE, MONENSIN,
PENCICLOVIR, PHOSPHONOACETIC ACID, PHOSPHONOFORMIC ACID,
RIBAVIRIN, SINEFUNGIN, THIOSEMICARBAZONES, TRIFLUOROTHYMIDINE, TUNICAMYCIN, VALACICLOVIR, ZANAMIVIR. [See also Book
ref. 134.]
AOAC Association of Official Analytical Chemists (of the USA).
AOAC use-dilution test A CARRIER TEST (q.v.), devised by the
AOAC, which determines the USE-DILUTION of a given disinfectant.
To each of a number of dilutions of the disinfectant is added a
(contaminated) small steel carrier; after immersion for 10 min,
each carrier is transferred to broth to detect any surviving
microorganisms. Sporicidal activity is determined by exposing
the endospores of Bacillus subtilis ATCC 19659 or Clostridium
sporogenes ATCC 9081 to the disinfectant and subsequently
testing for viability.
AP endonuclease See BASE EXCISION REPAIR.
AP site An apyrimidinic or apurinic site in DNA (see ADAPTIVE
RESPONSE and URACIL-DNA GLYCOSYLASE).
6-APA 6-AMINOPENICILLANIC ACID.
ApaI See RESTRICTION ENDONUCLEASE (table).
apalcillin A penicillin (see PENICILLINS) which is active against
both Gram-positive and Gram-negative bacteria (including Pseudomonas aeruginosa) [AAC (1982) 21 906911].
Apc APHIDICOLIN.
aperture diaphragm See CONDENSER.
APES See AAS.
APH Aminoglycoside phosphotransferase (see AMINOGLYCOSIDE
ANTIBIOTICS).
Aphanizomenon A genus of filamentous CYANOBACTERIA; the
cells are cylindrical with closely abutting ends, and the filaments
45
Aphanoascus
Coniophoraceae. Basidiocarp: characteristically resupinate;
basidiospores: pigmented, with a cyanophilic spore wall. Genera:
e.g. CONIOPHORA, Gyrodontium, and SERPULA.
Corticiaceae. Basidiocarp: characteristically resupinate or
effused-reflexed, with a hymenium that may be e.g. smooth or
wrinkled. Genera: e.g. Botryobasidium, Christiansenia (see also
MYCOPARASITE), Merulius, Mycoacia, Peniophora (see also HETEROBASIDION), Phanerochaete (see also WHITE ROT and LIGNIN),
and Phlebia.
Fistulinaceae. Basidiocarp: annual, pileate with a lateral stipe,
fleshy and moist; the hymenophore consists of a layer of closely
packed parallel tubules. Fistulina hepatica (the edible beefsteak fungus) causes BROWN OAK. It forms a fan-shaped or
tongue-shaped basidiocarp whose upper surface is rusty brown,
and whose lower (hymenial) surface is pale yellow when
unbroken; the reddish monomitic context of the pileus exudes a
red liquid when cut.
Ganodermataceae. Basidiocarp: annual or perennial, typically
fan-shaped and horizontal, either non-stipitate or borne on a
lateral stipe; the context of the pileus is trimitic, and the underside of the pileus bears a porous hymenophore. Basidiospores:
ovoid, typically flattened at one pole; ornamentations on the
inner, brown layer of the spore wall penetrate deeply into the
outer, hyaline layer of the spore wall. The organisms occur e.g.
on felled timber; Ganoderma applanatum causes heart rots in
various types of tree, infection occurring via wounds.
Hydnaceae. Basidiocarp: typically mushroom-shaped, with a
monomitic, non-xanthochroic context; the hymenophore consists
of a layer of pendulous tooth-like processes (spines or teeth)
on the underside of the pileus. Basidiospores: non-pigmented,
spheroidal. Hydnum repandum (the hedgehog fungus) is an
edible species which forms a thick, commonly cream-coloured
pileus and a short, thick stipe which is often eccentrically located
on the pileus; the teeth are often decurrent.
Hymenochaetaceae. Basidiocarp: annual or perennial, ranging
from resupinate to pileate or clavate according to species;
hymenophore: poroid (in e.g. INONOTUS and Phellinus) to smooth
(in Hymenochaete). Basidiospores: pigmented or colourless. The
organisms are commonly lignicolous.
Polyporaceae. Basidiocarp: annual or perennial, ranging (with
species) from resupinate to pileate (either stipitate or sessile);
the context is non-xanthochroic, and (according to species) may
be mono-, di- or trimitic, and e.g. corky, leathery or woody.
The hymenophore is typically porous, the hymenium being
confined to the walls of the pores. (cf. LENTINUS, PLEUROTUS.)
Basidiospores: colourless and usually smooth. The organisms
grow on felled timber and on living trees. Genera: e.g. CORIOLUS,
DAEDALEA, FOMES, Grifola, HETEROBASIDION, Irpex, Laetiporus,
LENTINUS, Lenzites, PIPTOPORUS, PLEUROTUS, POLYPORUS, PORIA,
Rigidoporus (see also BUTT ROT), TRAMETES and Tyromyces.
Schizophyllaceae. Basidiocarp: fan-shaped or lobed; basidiospores: colourless and smooth. The organisms are characteristically lignicolous. Genera: e.g. SCHIZOPHYLLUM.
Sparassidaceae. Basidiocarp: branching, flattened, monomitic
lobes, the hymenium being on both sides of the erect lobes.
Genera: e.g. SPARASSIS.
Stereaceae. Basidiocarp: appressed, effused-reflexed or stipitate, typically dimitic; basidiospores: colourless and smooth. The
organisms are characteristically lignicolous. Genera: e.g. Amylostereum (see also WOODWASP FUNGI), Chondrostereum (see also
SILVER LEAF), Podoscypha, STEREUM.
API system See MICROMETHODS.
apical Terminal: at the tip or distal part of a structure. Antonym:
basal.
apothecium
Some bacteria can induce apoptosis in host cells. Thus, for
example, on phagocytosis by a macrophage, Shigella can escape
from the vacuole and then induce apoptosis in the phagocyte by
means of a plasmid-encoded protein, IpaB. IpaB, secreted by
a type III secretory system (see PROTEIN SECRETION), activates
the host cells IL-1b-converting enzyme (ICE, see INTERLEUKIN1); activated ICE (i) initiates apoptosis in the macrophage, and
(ii) activates the intracellular, inactive form of IL-1b. Activated
IL-1b, when extracellular, may initiate an acute inflammatory
response (involving TNF-a, IL-1, IL-6 and IL-8). In one model
of shigellosis, these events have a positive role in promoting
a pro-inflammatory response that helps to control the infection
[TIM (1997) 5 201204].
The Shigella example (above) involves an endogenous stimulus (via the IpaB protein). Exogenous stimuli include the binding
of certain cytokines, or immune cells, to specific cell-surface
receptors on target cells. Thus, apoptosis is one of the possible
effects which may follow when tumour necrosis factor binds to
its receptor (see TNF). Induction of apoptosis by CD8+ T cells
may be possible in at least two different ways. One way involves
interaction between cell-surface molecules on the T cell and target cell (see FAS). Alternatively, following contact between T
cell and target cell, the T cell may release pore-forming lethal
agents (perforins) and also granzymes which are believed to
activate caspases (see below) in the target cell.
Whatever the stimulus that triggers apoptosis (in different
types of cell under differing conditions), it appears that the
mechanism of this process is dependent on certain intracellular cysteine proteases (caspases) that are synthesized as ZYMOGENS and activated specifically during apoptosis; these enzymes,
which have a cysteine residue at the active site, cleave specific protein substrates at a site adjacent to an aspartic acid
residue. The activity of a caspase on a substrate molecule may
lead to either inactivation or (less commonly) activation of the
given protein; for example, caspase-mediated activation of a
certain nuclease (caspase-activated DNase, CAD) leads to fragmentation of genomic DNA and formation of the characteristic
nucleosomal ladder. (CAD occurs in living cells, in inactive
form, complexed with an inhibitory entity referred to as ICAD.)
The activation of caspases appears to occur commonly by
proteolytic cleavage of the zymogen form, and, in at least some
cases, one caspase may be activated by an upstream caspase
in a caspase cascade. An understanding of the mechanism(s)
involved in caspase activation is central to an appreciation of the
process of apoptosis, and this area is being actively researched.
[Programmed cell death (concept, mechanism and control):
Biol. Rev. (1992) 67 287319. Apoptosis (reviews on biochemistry and other aspects of the process): Nature (2000) 407
770816.]
aporepressor See OPERON.
Aporpium See TREMELLALES.
Apostomatida See HYPOSTOMATIA.
aposymbiotic Refers to an organism (aposymbiont) which has
lost symbionts it normally possesses.
apothecioid Of an ASCOCARP: having, at maturity, a hymenium
more or less open to the environment as in a typical APOTHECIUM; apothecioid ascocarps may be e.g. cup-shaped, discoid
(circular and flat), or lirelliform (see LIRELLA).
apothecioid pseudothecium See ASCOSTROMA.
apothecium A typically dish- or cup-shaped or discoid, sessile
or stipitate ASCOCARP, the inner (or upper) surface of which is
lined with a hymenial layer of asci (often interspersed with
paraphyses); the main structural tissue of the apothecium is
AP-PCR
aprotinin A basic polypeptide which inhibits many serine PROTEASES, including e.g. trypsin, chymotrypsin, and some bacterial
proteases.
APS Adenosine-5 -phosphosulphate (also called adenosine-5 sulphatophosphate or adenylylsulphate). See ASSIMILATORY SULPHATE REDUCTION and DISSIMILATORY SULPHATE REDUCTION.
NH2
N
O
O
5
CH2
H
H
H
3
OH
OH
arboricolous
darker with age. The cell contains two nuclei. Slender lobopodia
are extended through a ventral aperture and are used chiefly for
feeding. A gas-filled vacuole may be formed in the cytoplasm
and apparently aids in the orientation of the organism. A. dentata
has a test bearing lateral spines, giving it a stellate appearance
when viewed from above. Arcella spp occur among vegetation
in ponds, in soil, etc.
Arcellinida An order of freshwater and soil amoebae (class
LOBOSEA) in which the cell is surrounded by a TEST which may
be primarily organic or primarily inorganic in composition, and
which is perforated by a single aperture through which pseudopodia can be extended. The cells commonly contain two or
more nuclei. Reproduction occurs asexually e.g. by binary fission. Genera include e.g. ARCELLA, Centropyxis, COCHLIOPODIUM,
DIFFLUGIA.
Archaea A DOMAIN of prokaryotic organisms which are evolutionarily distinct from members of the domain BACTERIA [see e.g.
JB (1994) 176 16]. These organisms were formerly classified
in the kingdom Archaebacteria, being distinguished from other
prokaryotes (kingdom Eubacteria) on the basis of e.g. nucleotide
sequences in 16S rRNA; later, the distinction between these two
groups of prokaryotes was deemed to be more fundamental than
previously supposed, and each kingdom was elevated to the taxonomic rank of domain.
Many archaeans are associated with environments characterized by e.g. high temperatures or high salinity, and such
organisms have been referred to as extremophiles. Nevertheless,
some archaeans are found in moderate environments such as
soil [e.g. PNAS (1997) 94 277282]. [Archaeal dominance in
the mesopelagic zone of the Pacific Ocean: Nature (2001) 409
507510.]
The domain Archaea has been divided into the kingdoms Euryarchaeota and Crenarchaeota. Euryarchaeota includes
halophiles (e.g. HALOBACTERIUM) and METHANOGENS. Crenarchaeota includes sulphur-dependent species such as DESULFUROCOCCUS and SULFOLOBUS.
Archaeans differ from bacteria in many ways. For example,
gene expression (transcription and translation) appears to be
closer to the eukaryotic pattern than the prokaryotic pattern
[TIM (1998) 6 222228]. The archaeal DNA-dependent RNA
POLYMERASE resembles more closely the eukaryotic (nuclear)
polymerase than the bacterial enzyme. Elongation factors in protein synthesis are (unlike their bacterial counterparts) sensitive
to DIPHTHERIA TOXIN. [Assembly of the archaeal signal recognition particle from recombinant components: NAR (2000) 28
13651373.]
[Replication origin of archaeans: TIBS (2000) 25 521523.]
At least some archaeal enzymes appear to have unique
structures [TIM (1998) 6 307314].
In some archaeans the cell wall may consist mainly or
solely of an S LAYER (q.v.) closely associated with the cytoplasmic membrane. The cell wall in some species contains
a peptidoglycan-like polymer, PSEUDOMUREIN (which is not
cleaved by the enzyme LYSOZYME).
The cytoplasmic membrane contains lipids of a type which
do not occur in species of Bacteria. In contrast to the esterlinked bacterial lipids, archaeal lipids are characteristically etherlinked molecules that contain e.g. isoprenoid or hydro-isoprenoid
components. Certain archaeal and bacterial lipids are structurally
analogous e.g. the di-ether and di-ester lipids, both types of
molecule having a single polar end. However, the archaeal
lipids also include other types such as tetra-O-di(biphytanyl)
diglycerol which contain two ether-linked glycerol residues,
arginine deiminase
arenaceous Resembling or (referring e.g. to the test of DIFFLUGIA)
incorporating or bearing grains of sand.
Arenaviridae (arenavirus group) A family of enveloped ssRNA
viruses. One genus: Arenavirus; type species: lymphocytic choriomeningitis virus (LCMV). LCMV has a worldwide distribution;
other arenaviruses are restricted to, and named after, particular geographical areas: Lassa virus, Mozambique (= Mopeia)
virus (probable member), and the New World arenaviruses
(the Tacaribe complex) Amapari (Brazil), Junn (Argentina),
Latino and Machupo (Bolivia), Parana (Paraguay), Pichinde
(Columbia), Tacaribe (Trinidad), and Tamiami (Florida, USA)
viruses. In the natural host (usually a single rodent species)
arenavirus infection is persistent and silent (see PERSISTENCE);
transmission occurs vertically and horizontally, apparently without involving vectors. Only LCMV, Lassa, Junn and Machupo
viruses cause significant human disease (see LASSA FEVER, LCM
VIRUS, VIRAL HAEMORRHAGIC FEVERS).
The arenavirus virion is spherical or pleomorphic, diam. ca.
50300 nm (average: 110130 nm). It consists of a lipoprotein
envelope enclosing a core of viral ribonucleoprotein (RNP) and
several host ribosomes (each 2025 nm diam.). The envelope is
derived from the plasma membrane of the host cell and bears
club-shaped, apparently hollow surface projections 510 nm
long [JGV (1983) 64 21572167]. There are two types of
viral ssRNA, designated L (3134S, MWt 2.13.2 106 ) and S
(2225S, MWt 1.11.6 106 ); the viral RNAs are complexed
with the major structural protein of the virion (N protein, p63)
to form a filamentous RNP nucleocapsid which has a beaded
appearance in the electron microscope and which forms noncovalently closed, supercoiled circles of various sizes [JGV
(1983) 64 833842]. The viral RNA is usually described as
negative-sense, but certain viral proteins are apparently encoded
by +ve-sense sequences in the genome see AMBISENSE RNA;
thus, e.g., the viral N protein is encoded by a sequence
complementary to the 3 -half of the S RNA, while the viral
glycoproteins are synthesized from a sequence corresponding
to the 5 -half of the S RNA. A non-glycosylated protein with
RNA-dependent RNA polymerase activity has been found in
virions of Pichinde virus. Arenavirus virions can be inactivated
by temperatures > 56 C, by pH <5.5 or >8.5, and by organic
solvents or detergents.
Arenaviruses can replicate in a wide range of mammalian
cell cultures (e.g. BHK-21, Vero and L cells). Virus replication occurs in the cell cytoplasm; the virus matures by budding
through the plasma membrane, when ribosomes become incorporated in the virion.
Arenavirus See ARENAVIRIDAE.
areolate Divided up into small areas (areolae). (Used e.g. of a
lichen thallus: see e.g. RHIZOCARPON.)
arg-poly(asp) Syn. CYANOPHYCIN.
arg regulon See ARGININE BIOSYNTHESIS.
Argentinian haemorrhagic fever A VIRAL HAEMORRHAGIC FEVER
caused by the Junn virus (see ARENAVIRIDAE). Mortality: usually
ca. 315%.
argentophilic Staining well with SILVER STAINS.
L-arginine biosynthesis See Appendix IV(a). In Escherichia coli
the genes encoding enzymes for arginine biosynthesis constitute
a REGULON (the arg regulon); four of the genes occur in a cluster
(argECBH ), the remainder occur singly at loci scattered around
the chromosome. [Biosynthesis and metabolism of arginine in
bacteria: MR (1986) 50 314352.]
arginine decarboxylase test See DECARBOXYLASE TESTS.
arginine deiminase See ARGININE DIHYDROLASE.
one at each end of the molecule; such molecules, which have two
polar ends, may span the width of the cytoplasmic membrane.
[Protein translocation across the archaeal cytoplasmic membrane: FEMS Reviews (2004) 28 324.]
The archaeal flagellum is markedly different in composition,
structure and apparent mode of assembly from that found
in bacteria. For example, the subunit, flagellin, is typically
glycosylated, and it contains a signal sequence (see SIGNAL
HYPOTHESIS) suggesting passage into/through the cytoplasmic
membrane (cf. bacterial flagellin, which passes through the
hollow structures of the developing flagellum); this latter feature
(as well as certain similarities between archaeal flagellins and
bacterial type 4 fimbriae) suggests that archaeal flagella assemble
from the base (in contrast to tip growth in bacteria) [JB (1996)
178 50575065]. The archaeal flagellar filament is typically
much thinner than the bacterial filament.
Various similar or analogous proteins have been found in
archaeans and bacteria. For example, the archaeal RadA protein
is apparently analogous to the RecA protein in bacteria [GD
(1998) 12 12481253]. Again, an FtsZ protein occurs in
members of both domains, suggesting that the cell division
apparatus was similar in a common ancestor [Mol. Microbiol.
(1996) 21 313319]. [The CELL CYCLE in archaeans: Mol.
Microbiol. (2003) 48 599604.]
archaean A member of the domain ARCHAEA. The term is also
spelt archaeon.
Archaebacteria A kingdom (now obsolete) which included all
those prokaryotes not classified in the kingdom EUBACTERIA.
[Phylogeny of the Archaebacteria: SAAM (1985) 6 251256.]
Some archaebacteria were placed in a separate taxon, Eocyta,
on the basis of ribosomal characteristics [PNAS (1984) 81
37863790]. (See also EOCYTES.) Members of the Archaebacteria are now included in the domain ARCHAEA.
Archaeobacteria A proposed class of prokaryotes (see MENDOSICUTES) corresponding to the (later) kingdom ARCHAEBACTERIA
(now also obsolete).
Archangium See MYXOBACTERALES.
archicarp In ascomycetes: the cell(s) which give rise to a fruiting
body or to a part of it.
archigregarines See GREGARINASINA.
Arcobacter A genus of Gram-negative, asporogenous bacteria
of the family Campylobacteraceae. Cells: spiral rods with
unsheathed flagella. Catalase +ve. Nitrate is reduced. Typically
urease ve. These organisms resemble Campylobacter spp
but differ e.g. in their ability to grow in air at 1525 C.
A. butzleri and A. cryophilus have been isolated from patients
with diarrhoea, including children in the developing countries;
most strains do not hydrolyse hippurate but do hydrolyse indoxyl
acetate.
arcuate Curved like a bow; arched.
Arcyria A genus of slime moulds (class MYXOMYCETES) which
form stalked, globose to cylindrical sporangia; the peridium is
evanescent, and the spores in masses may be yellow, pinkish,
red, etc. A. cinerea is common on dead wood and humus.
ARD Acute respiratory disease: a general term for any such
disease affecting closed populations of people (e.g. military
recruits, school children). Major causal agents of ARDs are
adenoviruses (usually Ad3, Ad4, Ad7, Ad14, or Ad21 see
MASTADENOVIRUS); an incubation period of ca. 57 days is
followed by fever, chills, headache, malaise and coryza, but
the disease is usually mild and self-limiting. A live vaccine,
administered orally in enteric-coated capsules, is widely used
for preventing adenoviral ARD in military recruits.
51
arginine dihydrolase
arginine dihydrolase (ADH) An enzyme system which catalyses the catabolism of arginine, with a concomitant substrate-level
phosphorylation; the system occurs in a range of bacteria. (i)
Arginine deiminase hydrolyses arginine to citrulline and ammonia. (ii) Ornithine carbamoyltransferase catalyses a phosphorolytic cleavage of citrulline to form carbamoyl phosphate and
ornithine. (iii) Carbamate kinase transfers the phosphate group
of carbamoyl phosphate to ADP to form ATP and carbamic acid,
the latter dissociating spontaneously to CO2 and NH3 .
Tests for ADH production are widely used in the identification
of certain bacteria (e.g. members of the ENTEROBACTERIACEAE).
Typically, the organism is grown in a medium containing Larginine and a pH indicator; the presence of ADH is indicated
by an alkaline reaction after a few days incubation. [Methods:
Book ref. 2, pp. 411412.]
arg-poly(asp) Syn. CYANOPHYCIN.
argT gene See BINDING PROTEIN-DEPENDENT TRANSPORT SYSTEM.
Argyn See SILVER.
Argyrol See SILVER.
argyrome Syn. SILVER LINE SYSTEM.
argyrophilic Syn. ARGENTOPHILIC.
arildone (4-[6-(2-chloro-4-methoxyphenoxy)-hexyl]-3,5-heptanedione) An ANTIVIRAL AGENT which is active against various
DNA and RNA viruses in vitro; it blocks uncoating in polioviruses and apparently also in herpes simplex viruses. Arildone
may be useful clinically e.g. in the topical treatment of HERPES
SIMPLEX infections.
Arizona See SALMONELLA.
arizonosis A POULTRY DISEASE, caused by Salmonella arizonae
(= Arizona hinshawii), characterized by malaise, diarrhoea, and
often symptoms of CNS involvement.
Arkansas bee virus See NODAVIRIDAE.
ArlSArlR See TWO-COMPONENT REGULATORY SYSTEM.
Armillaria (Armillariella)
A genus of mainly lignicolous
fungi (AGARICALES, Tricholomataceae). A. mellea (the honey
fungus) grows saprotrophically on many types of wood, forms
a symbiotic association with certain orchids (see MYCORRHIZA),
and is parasitic on a range of deciduous and coniferous trees,
on certain shrubs, and on some herbaceous plants. The fruiting
body is highly variable in colour and appearance, the pileus
being convex to flat (ca. 315 cm diam.), ochre to brown,
with darker scales particularly near the centre; the upper part
of the stipe, which often bears a wide annulus, is initially
whitish, later reddish-brown. Basidiospores: ca. 89 56 m.
The fruiting bodies (which exhibit BIOLUMINESCENCE) typically
occur in clusters. The organism spreads by means of tough, black
RHIZOMORPHS (boot laces) which may be found e.g. under the
bark of infected trees or in soil. (See also CARBON DISULPHIDE
and THREITOL.)
Armillariella See ARMILLARIA.
armoured dinoflagellates See DINOFLAGELLATES.
aroA gene See STAPHYLOCOCCUS (S. aureus).
arogenate See AROMATIC AMINO ACID BIOSYNTHESIS.
aroH gene See TRP OPERON.
aroma bacteria See DIACETYL.
aromatic amino acid biosynthesis Phenylalanine (Phe), tyrosine (Tyr) and tryptophan (Trp) are synthesized via the shikimate pathway: Appendix IV(f). Although most of the steps in
this pathway are apparently more or less universal, the control
mechanisms and physical organization of the enzymes (e.g. the
formation of multienzyme complexes) vary between species and
may be useful taxonomic criteria [CRM (1982) 9 227252].
The reactions by which prephenate is converted to Phe and Tyr
Ascetospora
brucellosis, gonorrhoea, Haverhill fever, Lyme disease, rickettsioses, syphilis, tuberculosis, yaws; it may also be caused
by certain viruses e.g., parvovirus [Lancet (1985) i 419421,
422425], Ross River virus, rubella virus. Septic arthritis is
due to infection of the synovial fluid commonly by staphylococci e.g. secondarily to OSTEOMYELITIS in an adjacent bone,
or as a complication of septicaemia; S. epidermidis may cause
chronic septic arthritis of the hip following total hip replacement.
(See also RHEUMATOID ARTHRITIS and REITER SYNDROME.)
Arthroascus A genus of fungi (family SACCHAROMYCETACEAE)
which form yeast cells (which bud, often bipolarly, on a
wide base) and true mycelium (which tends to break up into
arthrospores). Asci are formed directly after conjugation between
two cells. Non-fermentative; NO3 is not assimilated. Species:
A. javanensis, isolated e.g. from soil, fruit, rotting wood. [Book
ref. 100, pp. 114116.]
Arthrobacter A genus of obligately aerobic, catalase-positive,
asporogenous bacteria (order ACTINOMYCETALES, wall type
VI see also PEPTIDOGLYCAN) which occur in the soil. In culture
the organisms initially grow as irregular, lumpy, pleomorphic
rods, with or without primary branching, but stationary-phase
cultures consist predominantly of spherical or ovoid cells;
on subculture rod-shaped forms develop. Optimum growth
temperature: ca. 25 C. Arthrobacter spp have an oxidative-type
metabolism; they are not cellulolytic. GC%: ca. 5966. Type
species: A. globiformis.
Arthrobotrys A genus of fungi of the HYPHOMYCETES. Species
can grow saprotrophically and can trap and digest nematodes
(see NEMATOPHAGOUS FUNGI); A. oligospora can also attack and
kill other fungi [FEMS Ecol. (1985) 31 283291].
arthroconidium Syn. ARTHROSPORE.
Arthrocystis See EIMERIORINA.
Arthroderma A genus of fungi of the GYMNOASCALES (anamorphs:
CHRYSOSPORIUM; Trichophyton).
arthrospore (arthroconidium) (1) An arthric CONIDIUM. (2) Any
CONIDIUM formed by thallic conidiogenesis.
Arthuria See UREDINIOMYCETES.
Arthus reaction A severe local inflammatory skin reaction which
involves a TYPE III REACTION; the reaction becomes maximal
312 hours after the intradermal administration of antigen, and
involves erythema, oedema, and local haemorrhage and necrosis.
Arthus-type reaction Any disorder, other than the classical
ARTHUS REACTION, which involves a TYPE III REACTION see e.g.
FARMERS LUNG and GLOMERULONEPHRITIS.
artichoke curly dwarf virus See POTEXVIRUSES.
artichoke mottled crinkle virus See TOMBUSVIRUSES.
artifact Syn. ARTEFACT.
Artogeia rapae GV See BACULOVIRIDAE.
ARV See HIV.
arylsulphatase An enzyme which can hydrolyse aromatic sulphate esters at the OS bond; arylsulphatases occur e.g. in some
Aspergillus and Mycobacterium spp.
arylsulphatase test A test used in the identification of Mycobacterium spp. Essentially, the test strain is grown in a liquid
medium containing tripotassium phenolphthalein disulphate
(TPD); ARYLSULPHATASE-positive strains cleave TPD to PHENOLPHTHALEIN which is detected by a colour change on addition of
alkali after 10 days (for slow-growing strains) or after 3 or 7
days (for rapidly-growing strains).
ascarylose 3,6-Dideoxy-b-L-mannopyranose: a sugar found e.g.
in the LIPOPOLYSACCHARIDE of certain strains of Yersinia pseudotuberculosis (and in the eggs of Ascaris worms).
Ascetospora A phylum of PROTOZOA [JP (1980) 27 3758]
which form spores containing one or more sporoplasms but
Melarsoprol (a derivative of benzenearsenous acid a trivalent arsenical) is effective against both West and East African
strains of the causal agent of sleeping sickness (Trypanosoma
brucei gambiense and T. brucei rhodesiense, respectively).
The specific target of the drug is trypanothione (N 1 ,N 8 bis[glutathionyl]spermidine) [PNAS (1989) 86 26072611].
Melarsoprol reacts with trypanothione to form an adduct (Mel T)
which inhibits trypanothione disulphide reductase an enzyme
essential for regulating the parasites thiol/disulphide balance.
Melarsoprol crosses the bloodbrain barrier less readily than
eflornithine, but it is still regarded as the most effective trypanocidal drug available for treating sleeping sickness [AP
(1994) 33 147].
Trypanosomes exposed sub-lethally to arsenicals develop
resistance quite readily, possibly owing to decreased uptake.
(b)(in energy metabolism) Some bacteria use arsenate (or
selenate) as electron acceptor in anaerobic respiration, electron
donors including e.g. acetate, lactate and ethanol (according
to species); cell-envelope reductases have been found [FEMS
Reviews (1999) 23 615627]. Arsenite is used as electron donor
in autotrophic CARBON DIOXIDE fixation and as a respiratory
electron acceptor [FEMS Ecol. (2004) 48 1527; JB (2004)
186 16141619].
ART Automated reagin test: a qualitative or quantitative STANDARD TEST FOR SYPHILIS similar in principle to the RPR TEST.
arteannuin Syn. QINGHAOSU.
artefact (artifact) Any feature which does not occur in a specimen under natural conditions, but which may be seen in that
specimen during experimentation. Artefacts are due to the disturbance introduced by the process of experimentation or observation; they may occur e.g. as a result of FIXATION.
artemether See QINGHAOSU.
artemisinine Syn. QINGHAOSU.
arteritis Inflammation of an artery or arteries.
Arterivirus
A genus of viruses (family TOGAVIRIDAE); the
arterivirus group currently includes LACTATE DEHYDROGENASE
VIRUS, SIMIAN HAEMORRHAGIC FEVER VIRUS, the Lelystad virus
(see BLUE-EARED PIG DISEASE) and equine arteritis virus.
In equines, equine arteritis virus causes necrosis of small
arteries with various clinical manifestations for example, rhinitis, oedema, enteritis, bronchopneumonia. Infection of pregnant
mares commonly results in abortion. Transmission occurs both
horizontally and vertically; vectors are unknown. The virus can
infect a range of vertebrate cells in vitro.
The viruses in this group are similar in their morphology and
genomic organization; moreover, all exhibit a predilection for
macrophages, and all tend to cause a lengthy period of viraemia.
artesunate See QINGHAOSU.
Arthonia See ARTHONIALES.
Arthoniales An order of fungi of the ASCOMYCOTINA; members
include crustose LICHENS (photobiont green, often trentepohlioid)
and lichenicolous and saprotrophic fungi. Ascocarps are APOTHECIOID and may be lirelliform, irregular, etc; they contain paraphysoids. Asci are bitunicate, usually clavate. Genera: e.g.
Arthonia.
Arthopyrenia A genus of crustose LICHENS of the order DOTHIDEALES; ascospores have one to several septa. A. halodytes (photobiont Hyella) is a marine species which grows endolithically
in calcareous rocks and on the shells of limpets, barnacles etc
in the intertidal zone; it occurs in Europe and N. America.
arthralgia Joint pain.
arthric conidium See CONIDIUM.
arthritis Inflammation of one or more joints. It may occur as a
symptom or complication of various infectious diseases e.g.
53
asepsis
Following plasmogamy, the events leading to ascus formation
vary according to species.
Ascus formation in ascogenous yeasts. After plasmogamy
(which may occur e.g. by the fusion of somatic cells or
ascospores), karyogamy commonly follows without delay. The
zygote may undergo MEIOSIS immediately (as e.g. in Schizosaccharomyces octosporus) so that the ascus develops directly from
the zygote; alternatively, meiosis may be delayed for one or
more mitotic divisions (e.g. as in the diploid budding phase
of Saccharomyces cerevisiae) in which case the ascus develops following meiosis in one of the diploid descendents of the
zygote. Following meiosis, the four (haploid) nuclei may develop
directly into four ascospores (as in e.g. S. cerevisiae) or there
may be subsequent mitotic division with the eventual formation
of e.g. eight ascospores (as in e.g. S. octosporus). The process
by which a nucleus gives rise to an ascospore is called free cell
formation (see below).
Ascus formation in other ascomycetes. (The following is
necessarily a generalized account since details of the process
vary from species to species.) After plasmogamy, karyogamy
is typically delayed. One or more hyphae (ascogenous hyphae)
arise from the ASCOGONIUM, and the (haploid) male and female
nuclei migrate into these hyphae. The tip of each hypha then
curves to form a crook (crozier ) such that two nuclei (one
from each parent) occur in the curved upper portion of the
crozier. These nuclei then undergo mitosis, simultaneously, with
their mitotic spindles arranged parallel to the long axis of
the ascogenous hypha; the subsequent formation of a septum
creates an apical cell (the ascus mother cell ) which contains
one daughter nucleus from each of the two original nuclei.
Karyogamy now occurs. The zygote undergoes meiosis followed
by one or more mitotic divisions to produce the number of
haploid nuclei (ascospore initials) characteristic of the species.
The ascospores develop by free cell formation. In this process,
each nucleus (with a portion of cytoplasm) becomes enclosed
within an envelope (the spore-delimiting membrane, SDM)
composed of two unit-type membranes. In some ascomycetes
(e.g. many members of the Endomycetales) the nucleus may
be enveloped directly by vesicles (derived from the GOLGI
APPARATUS or Golgi-equivalent?) which develop in association
with the SPINDLE POLE BODY. In other species, e.g., Taphrina
deformans and some species of Tuber, each nucleus becomes
enveloped by membrane derived from invaginations of the
ascus plasma membrane. However, in most euascomycetes
the SDMs derive from a system of nuclear and/or endoplasmic
reticular membranes which, initially, form a discontinuous layer
around the periphery of the ascus cytoplasm (the peripheral
membrane cylinder ). That portion of the ascus cytoplasm which
is not incorporated into ascospores is termed the epiplasm.
Ascospore wall material is subsequently laid down between the
two layers of the SDM. [Ascospore development: Book ref. 175,
pp. 107129.]
Types of ascus. There are at least nine morphologically
and/or functionally distinct types of ascus [Bot. J. Lin. Soc.
(1981) 82 1534 (2933)]: see e.g. ANNELATE ASCUS, BITUNICATE
ASCUS, OPERCULATE ASCUS, OSTROPALEAN ASCUS and PROTOTUNICATE ASCUS. (See also UNITUNICATE ASCUS and BILABIATE.)
ascus mother cell See ASCUS.
Asellariales See TRICHOMYCETES.
asepsis (1) The state in which potentially harmful microorganisms (e.g. pathogens in a medical context, spoilage organisms in
an industrial context) are absent from particular tissues, materials or environments; in this sense asepsis does not necessarily
aseptate
involve sterility (cf. STERILE (sense 1)). (2) A state of sterility.
(See also ANTISEPSIS and STERILIZATION.)
aseptate Lacking septa see SEPTUM.
aseptic (adj.) Refers to ASEPSIS (sense 1 or 2).
aseptic meningitis See MENINGITIS (b).
aseptic technique Precautionary measures taken to prevent the
contamination of cultures, sterile media etc and/or the infection
of persons, animals or plants by extraneous microorganisms.
Thus, e.g. all vessels for media etc must initially be STERILE (presterilized disposable petri dishes, syringes etc are often used).
The working surfaces of instruments (forceps, LOOPS etc), and
the rims of bottles used for dispensing sterile (non-flammable)
materials, are sterilized by FLAMING. Before use, sterile material
should not be exposed to non-sterile material or conditions. The
risk of contamination is reduced by treating bench surfaces
etc with DISINFECTANTS and/or with ultraviolet radiation (see
STERILIZATION). Procedures (e.g. INOCULATION) are carried out
in such a way that exposure to the atmosphere is reduced to
a minimum, or is eliminated (see e.g. SAFETY CABINET).
Ashbya See METSCHNIKOWIACEAE and STIGMATOMYCOSIS; see also
RIBOFLAVIN.
AsiA See ANTI-SIGMA FACTOR.
Asian flu See INFLUENZAVIRUS.
Asiatic cholera Syn. CHOLERA.
ASLT ANTISTREPTOLYSIN O TEST.
ASO test ANTISTREPTOLYSIN O TEST.
ASOT ANTISTREPTOLYSIN O TEST.
L-asparaginase (L-asparagine aminohydrolase; EC 3.5.1.1) An
enzyme which hydrolyses L-asparagine to L-aspartate and NH3 .
L-Asparaginase (e.g. from Escherichia coli or Citrobacter
sp) is used as an anticancer agent e.g. for treating acute
lymphocytic leukaemia in which the cancer cells require
exogenous asparagine. (See also ENZYMES.)
L-asparagine biosynthesis See Appendix IV(d).
asparenomycins CARBAPENEM antibiotics.
aspartame L-Aspartyl-L-phenylalanine methyl ester; it is used as
a sweetener in certain foods and beverages.
aspartase See ASPARTATE BIOSYNTHESIS.
aspartate ammonia-lyase See ASPARTATE BIOSYNTHESIS.
L-aspartate biosynthesis For the main pathway of aspartate
biosynthesis see Appendix IV(d). In many microorganisms,
aspartate can also be produced from fumarate and ammonia by
the enzyme aspartase (L-aspartate ammonia-lyase, EC 4.3.1.1),
but this (reversible) reaction is probably more important in the
deamination of aspartate than in its synthesis. (cf. IMMOBILIZATION sense 1.)
aspartokinase See Appendix IV(d).
aspergillic acid An antibiotic (a pyrazine derivative) formed by
Aspergillus flavus.
aspergilloma See ASPERGILLOSIS.
aspergillosis Any disease of man or animals in which the causal
agent is a species of ASPERGILLUS.
In man, the causal agent is usually A. fumigatus, although
A. flavus, A. niger or A. terreus may be involved. Infection
usually occurs by inhalation of air-borne conidia, but may
occur via wounds or by ingestion. The disease may be noninvasive, the fungus colonizing a pre-existing lung cavity (e.g.
a lung cyst or healed tuberculosis lesion) and forming compact
mycelial masses called aspergillomas (cf. MYCETOMA sense 2);
symptoms may be absent or may include chronic productive
cough and haemoptysis. Less commonly, the disease may
become invasive, disseminating to other organs (particularly in
immunocompromised patients); this form is commonly fatal.
Astrephomene
forming a parallel-sided columnar spore mass which may reach
ca. 1 mm in length. A. fumigatus has been reported to grow at
50 C. (See also FUMAGILLIN.)
A. phialiseptus is morphologically similar to A. fumigatus,
but it forms septate phialides which are longer than those of
A. fumigatus.
Aspidisca
A genus of ciliate protozoa (order HYPOTRICHIDA)
related to Euplotes but differing e.g. in typically having a
relatively reduced oral ciliature; species occur in freshwater and
marine habitats, and e.g. in some SEWAGE TREATMENT plants.
aspirin See PROSTAGLANDINS.
asporogenous Not capable of forming spores.
assay host (plant virol.) Syn. LOCAL LESION host.
assimilatory nitrate reduction The (typically aerobic) reduction of nitrate to ammonia, the ammonia being assimilated as
a source of nitrogen (see AMMONIA ASSIMILATION); nitrate can
be used as the sole source of nitrogen by many bacteria, various fungi, and most algae and plants. Nitrate is initially reduced
to nitrite typically by a soluble, oxygen-insensitive enzyme
(assimilatory nitrate reductase) in a reaction in which the electron donor may be a reduced pyridine nucleotide or a reduced
ferredoxin; in fungi the electron donor is often (sometimes
specifically) NADPH, but in e.g. Candida nitratophila it can
be either NADH or NADPH [JGM (1986) 132 19972003].
The assimilatory reduction of nitrate to nitrite does not generate proton motive force cf. DISSIMILATORY NITRATE REDUCTION.
Nitrite is reduced to ammonia by an assimilatory nitrite reductase, reducing power being derived (according to organism) from
NADPH, NADH or reduced ferredoxin commonly the latter
in algae and higher plants. The synthesis/activity of enzymes
involved in assimilatory nitrate reduction is regulated at least
partly by the extracellular concentrations of ammonia and nitrate.
assimilatory sulphate reduction Sulphate can be used as the
sole source of sulphur by most microorganisms. The major
assimilatory pathway in bacteria and fungi is shown in the
figure. (cf. DISSIMILATORY SULPHATE REDUCTION; see also SULPHUR
CYCLE.)
Astasia See EUGLENOID FLAGELLATES.
astaxanthin See PHAFFIA.
asteltoxin A polyene MYCOTOXIN isolated from toxic maize meal
cultures of Aspergillus stellatus (= A. variecolor, Emericella
variecolor ). In experimental animals asteltoxin can cause e.g.
paralysis of hind-limbs and respiratory impairment.
aster (cell biol.) See MITOSIS.
aster yellows See YELLOWS.
Asterionella
A genus of freshwater and marine planktonic
pennate DIATOMS. A. formosa occurs e.g. in lakes and reservoirs,
forming blooms in spring and, to a lesser extent, in autumn. In
this and other species each individual vegetative cell is long and
narrow with slightly flared ends; a variable number of cells (ca.
8 under optimum conditions) form a star-shaped colony in which
each corner of one end of a given cell is joined to one corner of
a neighbouring cell.
Asticcacaulis A genus of chemoorganotrophic, strictly aerobic
PROSTHECATE BACTERIA; habitat and life-cycle are similar to those
of CAULOBACTER, but one or more prosthecae arise subpolarly
and/or laterally and do not have an adhesive role adhesive
material occurring on the cell surface.
Astomatida An order of protozoa (subclass HYMENOSTOMATIA) in
which the cells are typically large or long, are uniformly ciliated,
contain a number of contractile vacuoles, lack a cytoproct,
and are invariably mouthless; some species have an elaborate
holdfast organelle. Asexual reproduction may involve budding
SO4
ATP
sulphate
adenylyltransferase
PPi
APS
ATP
APS
kinase
ADP
PAPS
+
NADPH + H
FAD
thiol
PAPS
reductase
NADP
PAP
SO3
+
3NADPH + 3H
sulphite
reductase
+
3NADP
3H2O
S2
ASSIMILATORY SULPHATE REDUCTION in bacteria and fungi.
APS = adenosine-5 -phosphosulphate (see APS); PAPS = 3 -phosphoadenosine-5 -phosphosulphate; PAP = 3 -phosphoadenosine5 -phosphate. The pathway for the assimilation of sulphide depends
on organism. In e.g. Escherichia coli sulphide is incorporated into
O-acetylserine to form cysteine [Appendix IV(c)]. In e.g. Yarrowia
(Saccharomycopsis) lipolytica sulphide may be incorporated into
O-acetylserine (to form cysteine) or into O-acetylhomoserine to
form homocysteine; homocysteine may be converted to methionine [Appendix IV(d)] or (via cystathionine) to cysteine [see e.g. MGG
(1979) 174 3338].
Astrolophus
atovaquone See MALARIA.
Atoxoplasma
A genus of protozoa (suborder EIMERIORINA)
similar to LANKESTERELLA but parasitic in birds. [Book ref. 18,
p.13.]
atoxyl See ARSENIC.
ATP Adenosine 5 -triphosphate (see figure). (See also NUCLEOTIDE.) In both prokaryotic and eukaryotic cells ATP actively
participates in a range of processes and reactions which involve
the conversion or expenditure of energy (see also ATPASE); energy
derived from chemotrophic or phototrophic metabolism holds
the massaction ratio of the reaction (ATP ADP + Pi) at
values such that ATP hydrolysis is thermodynamically highly
favourable, i.e., it can yield free energy which the cell can use
for specific purposes. (See also ADENYLATE ENERGY CHARGE.)
NH2
N
N
O
O
O
O
O
O P
O CH2
4
N
O
OH
OH
aurintricarboxylic acid
ALPHAHERPESVIRINAE).
aurodox
aurodox See POLYENE ANTIBIOTICS (b).
aurovertins A group of polyene, a-pyrone-containing MYCOTOXINS isolated from cultures of Calcarisporium arbuscula.
[Biosynthesis: PAC (1986) 58 239256.] Aurovertins bind noncovalently to, and inhibit, (F0 F1 )-type PROTON ATPASES.
Australia antigen HBsAg: see HEPATITIS B VIRUS.
Australia X disease Syn. MURRAY VALLEY FEVER.
Australian bat lyssavirus See LYSSAVIRUS.
auto-agglutination (saline agglutination) Spontaneous agglutination which may occur when bacterial cells (or other particulate
materials) are suspended in e.g. saline. (See also VW ANTIGENS.)
auto-a Syn. ALPHA PEPTIDE.
autoantibody An ANTIBODY produced by an individual against
one of its own antigens. (See e.g. TYPE V REACTION.)
autoantigen An antigen homologous to an AUTOANTIBODY.
Autobiocounter M 4000 See HACCP.
autocatalytic splicing See SPLIT GENE (b, c and e).
autochthonous (1) Indigenous to a given environment. (cf.
ALLOCHTHONOUS.) In a given environment the autochthonous
microorganisms maintain more or less constant numbers or
A
E
chamber
F
D
steam inlet
275-550 kPa
(40-80 lb/inch2)
H
G
J
K
steam/condensate
outlet
AUTOCLAVE. Simplified, diagrammatic representation of a Series 225 steammains autoclave (courtesy of Baird and Tatlock (London) Ltd).
A. Steam inlet valve. The valve is opened/closed electromagnetically its operation being governed by the pressure controller/indicator.
(Control by temperature via the thermocouple is an available option.) B. Pressure controller/indicator. C. Door microswitch a safety
device; electrical power is connected to the autoclave only when the microswitch has been actuated, i.e., when the door has been fully
closed. Additionally, this device automatically opens the steam exit valve if any attempt is made to open the door while the chamber is under
pressure. D. Door closure bolts which operate microswitches. E. Safety valve set to open at 275 kPa. F. Filters which prevent blockage
of steam discharge lines and steam trap. G. Thermocouple pocket: temperature control/indicator/recording option. H. Manually-operated
by-pass valve can be operated in case of electrical power failure. (Under such conditions valve J could not be opened.) The valve contains a
built-in bleed which permits a small but continual flow of steam from the chamber to the exterior. J. Electrically-operated steam exit valve. K.
Steam trap.
Operational sequence. 1. Insert load. 2. Secure door. 3. Set controls for required pressure/temperature and sterilizing time. 4. Switch on
power. Steam enters the chamber through A, and the downwardly-displaced air is purged, via filters F, through (a) the steam trap K and (b) the
permanent bleed H; J is closed, and when steam leaves the chamber, K closes. A closes when the chamber pressure reaches the selected
value. Steam continues to leave the chamber via the permanent bleed H permitting continual temperature monitoring by the thermocouple G;
since G is located at the lowest (and hence coolest) part of the system, it measures the worst case temperature the chamber temperature
always being higher than that registered by G. Sterilizing conditions within the chamber are maintained (against heat losses and against the
continual steam bleed) by periodically admitting a pulse of steam via A. At the end of the sterilization cycle steam is discharged from the
chamber via J; when atmospheric pressure has been re-established in the chamber the door can be opened and the load withdrawn.
Automatic timing of the sterilization cycle commences when the chamber pressure (or, optionally, temperature measured by G) reaches
the desired value.
60
autogamy
the entry of contaminated air is prevented by the presence of a
filter in the air intake line. In vacuum autoclaves steam can be
removed, and materials dried, by connecting a vacuum line to
the chamber.
Regular monitoring of an autoclaves performance is important; monitoring devices should be used to check the temperatures reached at a number of different locations within the chamber. Monitoring devices may be physical (e.g. thermocouples),
chemical (e.g. BROWNES TUBES), or biological (test envelopes
containing the endospores of e.g. Bacillus stearothermophilus).
In biological monitoring the autoclaved spores are tested for viability by attempting to culture them; although such a process is
directly related to the aim of autoclaving, it involves a builtin delay (i.e. the incubation time). (See also AUTOCLAVE TAPE;
BOWIEDICK TEST.)
Some materials (e.g. petroleum jelly, liquid paraffin) cannot be
sterilized by autoclaving owing to their impermeability to steam;
such materials (and e.g. clean glassware) are usually sterilized
in a HOT-AIR OVEN.
(See also CHEMICLAVE; LOW-TEMPERATURE STEAM DISINFECTION;
STEAMER; STERILIZER.)
autoclave tape Paper tape (usually self-adhesive) which changes
colour (or exhibits other visible changes) when exposed to
sterilizing conditions in an AUTOCLAVE. (See also BOWIEDICK
TEST.)
autocolony A colony (or coenobium) which develops within one
cell of a parent colony and which, when released, resembles the
parent colony (see e.g. SCENEDESMUS). (cf. AUTOSPORE.)
autocompartmentalization See PROTEASOME.
autocoupling hapten See HAPTEN.
autodigestion (of lamellae) See BASIDIOSPORES.
autodisplay (biotechnol.) Autotransporter-mediated display of
recombinant proteins at the cell surface of Escherichia coli. In
this method, the a domain of the AIDA-I autotransporter (see type
IV systems in PROTEIN SECRETION) is replaced by a recombinant
protein; this is done by preparing a fusion protein consisting
of the sequence encoding the b domain and that encoding the
(heterologous) recombinant protein. In one study, the a domain
was replaced e.g. by the cholera toxin B subunit; cells with the
(normal) outer membrane protease OmpT cleaved the (recombinant) a domain, which was released from the cell, but in
mutant (ompT ) cells, which lack a functional OmpT protease,
the subunit was not cleaved, but displayed at the cell surface.
[Autodisplay: JB (1997) 179 794804.]
autoecious Syn. HOMOXENOUS.
autofluorescence See FLUORESCENCE.
autogamy (self fertilization) In certain protozoa: a sequence of
events which culminates in the fusion of haploid nuclei or
gametes derived from a single cell; autogamy occurs e.g. in
certain ciliates (e.g. Paramecium but apparently not in e.g.
Tetrahymena) and in some sarcodines.
In Paramecium aurelia each of the two micronuclei undergoes meiosis; of the eight haploid pronuclei produced all except
one disintegrate. The surviving pronucleus divides mitotically
to form a pair of gametic nuclei; these nuclei subsequently
fuse to form the (homozygous) zygotic nucleus (= synkaryon).
Two mitotic divisions then occur; two of the resulting (diploid)
nuclei become new micronuclei, the other two become macronuclei the original macronucleus having disintegrated during the
preceding events. During the next binary fission one macronucleus passes to each daughter cell; both micronuclei divide,
mitotically, and a pair of micronuclei passes to each daughter cell thus re-establishing the normal nuclear constitution.
autogenous regulation
Since only the original complement of genes is involved, the
potential for genetic change in autogamy is less than that in
CONJUGATION; nevertheless, new combinations of alleles may be
formed during the meiotic divisions. (See also ACTINOPHRYS and
ACTINOSPHAERIUM.)
In some organisms autogamy occurs spontaneously; in others
it may be induced by starvation, ageing, radiation etc.
autogenous regulation (mol. biol.) The regulation of expression
of a gene or operon by its own product(s). (See e.g. RIBOSOME
(biogenesis).)
autogenous vaccine A VACCINE prepared by the culture and inactivation of pathogen(s) isolated from a patient and subsequently
used to inoculate that patient.
Autographa californica NPV See NUCLEAR POLYHEDROSIS
VIRUSES.
autoimmune disease Any disease directly attributable to AUTOIMMUNITY. In some autoimmune diseases (e.g. acquired haemolytic
anaemias) antibodies play a significant role, but many autoimmune diseases are cell-mediated. (See also e.g. MULTIPLE SCLEROSIS.)
autoimmunity An expression of IMMUNITY (1) in which the body
directs immunological mechanism(s) against one or more of its
own components. (See also TYPE V REACTION.)
autoinducer See AUTOINDUCIBLE ENZYME and QUORUM SENSING.
autoinducible enzyme A (repressible) enzyme whose induction
in a given organism is brought about by the presence of
a specific compound (autoinducer) that is produced by the
organism itself (cf. enzyme induction in e.g. the LAC OPERON).
An example is bacterial luciferase (see BIOLUMINESCENCE). In
this system autoinducer is secreted by the bacteria and can
accumulate to the critical, effective concentration (sufficient to
bring about derepression) only when the organisms are in a
confined environment (e.g. in the luminous organs of certain
marine fish).
autoinfection Infection resulting from the transfer of a pathogen
from one site to another in the same individual (cf. RE-INFECTION).
autologous (immunol.) Present in or derived from an individuals
own tissues.
autologous blood transfusion See TRANSFUSION-TRANSMITTED
INFECTION.
autolysate The products of AUTOLYSIS. (See e.g. YEAST EXTRACT.)
autolysin (autolytic enzyme) Any of a range of endogenous
enzymes which, by degradation of certain structural cell components (e.g. PEPTIDOGLYCAN in bacteria), can bring about AUTOLYSIS or AUTOPHAGY; autolysins are apparently involved in normal
processes of growth and development (e.g., spore germination;
cell wall polymer extension and cell separation during normal growth). Mutant bacteria defective in autolysin activity
may show e.g. abnormal growth forms (e.g. filaments) or resistance to antibiotics active against the wild-type. In prokaryotes,
autolysins occur in the cell wall or (in Gram-negative species)
in the periplasmic space, often as inactive precursors which are
activated e.g. by proteases (see also BILE SOLUBILITY); in eukaryotes autolysins are sequestered in LYSOSOMES.
autolysis The lysis of a cell due to the action of its AUTOLYSINS
usually following the death of the cell or tissue.
autolytic enzyme Syn. AUTOLYSIN.
automatic volumetric spore trap Syn. HIRST SPORE TRAP.
autonomously replicating sequence See ARS.
autophagy The digestion, by a eukaryotic cell, of some of its
own internal components e.g., during periods of starvation.
(See FOOD VACUOLE.)
autoplaque A plaque (in a bacterial lawn plate) which resembles
that caused by a lytic bacteriophage, but in which no phage can
avermectins
which catalyse particular stage(s) in the synthesis of essential
growth factor(s); such a block may involve (a) the complete
absence of enzyme; (b) the presence of normal enzyme in
subnormal amounts; (c) the presence of abnormal enzyme
which is devoid of or has lowered enzymic activity. (See also
SYNTROPHISM.)
Apparent auxotrophy may result e.g. from a defective TRANSPORT SYSTEM; thus, e.g. an organism may appear to be an auxotroph if it is unable to take up a substrate which is necessary
for the synthesis of an essential growth factor. (See also CRYPTIC
MUTANT.)
Isolation of auxotrophic mutants. Since auxotrophs have
nutritional requirements in excess of those of the corresponding
(prototrophic) wild-type strains, they cannot be isolated from
mixed auxotrophprototroph populations by common selective
culture methods.
In the limited enrichment method, a dilute suspension of
mutagenized cells is inoculated onto a minimal medium which
has been enriched with limiting amounts of nutrients; the
dilution is chosen such that isolated colonies are obtained
following incubation. Any auxotrophic cells which may be
present form colonies which quickly exhaust the nutrient supply
at their locations so that colony size is restricted; a colony
of prototrophic cells, which is not restricted by nutrient supply,
attains a greater size. Thus, small colonies may be presumed to
be those of auxotrophs.
In the delayed enrichment method, the mutagenized preparation of cells is first inoculated onto a minimal medium. A small
quantity of molten minimal agar is then layered onto the surface of the inoculated medium and allowed to set. The plate is
then incubated. Colonies are formed only by prototrophs, and
the positions occupied by these colonies are recorded. Finally,
complete medium is layered onto the surface of the plate and
allowed to set; the plate is then re-incubated. As nutrients diffuse into the minimal agar the auxotrophic cells begin to grow
and form colonies.
Auxotrophic mutants may also be isolated by a REPLICA
PLATING process.
Another method is based on the differing effects of PENICILLIN on growing and non-growing cells of certain (penicillinsensitive) organisms. If a well-washed mixture of auxotrophic
and prototrophic cells is suspended in a minimal medium with an
appropriate concentration of penicillin, the prototrophs are lysed
while the auxotrophs, being unable to grow, remain viable. The
suspension is then washed and is plated on a complete medium
to recover the auxotrophs. In this method it is essential that the
mutagenized cells be grown in a complete medium for several
cell-division cycles prior to penicillin treatment. This is essential
because the newly mutated cells contain the full complement of
enzymes etc found in the prototroph; only after several rounds
of cell division do the progeny cells exhibit a truly auxotrophic
phenotype. Only low concentrations of cells should be used in
this method since substances from the lysed cells may be used
as nutrients by the auxotrophs thereby rendering the latter susceptible to lysis by penicillin. (cf. STREPTOZOTOCIN.)
auxotype See AUXANOGRAPHIC TECHNIQUE.
avenacin A fluorescent polycyclic SAPONIN formed in the roots
of oat plants (Avena spp). Avenacin confers resistance, in Avena
spp, to many strains of Gaeumannomyces graminis (see TAKEALL); however, G. graminis var. avenae forms an extracellular
glycosidase which detoxifies the compound.
avermectins Macrolide-like antihelmintic agents, obtained from
Streptomyces avermitilis, which are active against various human
and animal parasites [AEM (2003) 69 12631269].
aversion zone
avian myeloblastosis virus See AVIAN ACUTE LEUKAEMIA VIRUSES
and MYB.
avian myeloblastosis virus reverse transcriptase See REVERSE
TRANSCRIPTASE.
avian myelocytomatosis virus See AVIAN ACUTE LEUKAEMIA VIRUSES.
avian pneumoencephalitis Syn. NEWCASTLE DISEASE.
avian reticuloendotheliosis viruses (REVs) A group of type
C avian retroviruses of the ONCOVIRINAE. The group includes
the replication-competent viruses duck infectious anaemia virus,
Trager duck spleen necrosis virus and chicken syncytial virus,
and the replication-defective, v-onc+ (v-rel + ) strain T virus
(REV-T) and its associated helper virus (REAV, = REV-A).
REVs are pathogenic in poultry (chickens, ducks, turkeys),
causing a range of (usually rapidly lethal) diseases: e.g. anaemia,
visceral reticuloendotheliosis, enlargement and necrosis of the
spleen, lymphomas, and infiltrative nerve lesions. REV-T and its
helper (REV-A) can be lethal in chickens within ca. 714 days
of infection; the REV-A component has been reported to induce
or activate a splenic suppressor cell population which inhibits the
proliferation of cytotoxic cells capable of lysing REV-T-induced
tumour cells [MS (1984) 1 107112].
avian sarcoma viruses (ASVs) A group of v-onc+ type C
retroviruses (subfamily ONCOVIRINAE) which, after a short latent
period, cause tumours in fowl and (sometimes) other animals.
The group includes ROUS SARCOMA VIRUS, Fujinami sarcoma
virus (which carries v-fps), and Yamaguichi-73 sarcoma virus
(which carries v-yes). (cf. FES.)
avian tubercle bacillus Mycobacterium avium.
avianized vaccine Any vaccine containing microorganisms
whose virulence for a given host has been attenuated by adaptation in live chicks and/or serial passage through chick embryos
(eggs). Attenuated organisms may or may not be inactivated
prior to use in a vaccine. The FLURY VIRUS is an avianized strain.
Avicel A commercial preparation consisting of ground microcrystalline (insoluble) CELLULOSE (average DP ca. 200); it is used e.g.
for determining the ability of an organism or enzyme to degrade
microcrystalline cellulose. (cf. CM-CELLULOSE.)
avidin A protein (MWt ca. 68000) present e.g. in the white of
raw hens eggs; the chicken avidin molecule consists of four
identical subunits, and it can bind non-covalently, but very
strongly four molecules of BIOTIN. (See also ABC IMMUNOPEROXIDASE METHOD; cf. STREPTAVIDIN.)
avidity (immunol.) The stability of the antibodyantigen complex formed when multivalent antigen and homologous antiserum are mixed. Avidity depends not only on the AFFINITY
of the individual determinant-combining site bonds but also on
the number of satisfied valencies of the antigens and antibodies
since, e.g., a complex in which two antigen molecules are linked
by two antibody molecules is disproportionately more stable than
a complex in which the two antigen molecules are linked by a
single antibody molecule.
Aviemore model See RECOMBINATION (figure 2).
Avipoxvirus (fowlpox subgroup) A genus of viruses of the CHORDOPOXVIRINAE which infect birds (see e.g. FOWL POX). Avipoxviruses are commonly transmitted (mechanically) by arthropod
vectors. Infected cells form lipid-rich A-type inclusion bodies;
haemagglutinin is not formed. Infectivity is ether-resistant.
Members are closely related serologically. Type species: fowlpox
virus; other members include canarypox, juncopox, pigeonpox,
quailpox, sparrowpox, starlingpox and turkeypox viruses. (See
also POXVIRIDAE.)
avirulence gene (avr gene) (plant pathol.) In a plant-pathogenic
microorganism: a gene which interacts, functionally, with a
Azolla
wavelength) are also formed during growth on solid media at
30 C. Enlarged, ovoid or pleomorphic, non-motile, capsulated
forms (C forms) may develop under certain conditions
(e.g. in old cultures). Metabolism is mainly respiratory, with
either oxygen or NO3 acting as terminal electron acceptor;
DENITRIFICATION occurs under microaerobic conditions. Glucose
or fructose may be fermented weakly. Disaccharides are
not metabolized. Oxidase +ve; catalase variable; phosphatase
+ve; indole ve; weakly pectinolytic. Optimum growth
temperature: 3537 C. Colonies on potato agar are typically
pink, often wrinkled, not slimy. NITROGEN FIXATION occurs
under microaerobic conditions; an uptake hydrogenase
(see NITROGENASE) is present, and A. lipoferum (but not
A. brasilense) can grow as an H2 -dependent lithoautotroph.
Aerobic growth can also occur in the presence of fixed nitrogen
(e.g. NH4 + , NO3 ). GC%: 6971. Type species: A. lipoferum
(formerly Spirillum lipoferum).
[Book ref. 22, pp. 94104.]
Azospirilla occur in soil, both free-living and in association
with the roots of grasses (including cereals) and tuberous plants;
the bacteria occur on the root surface, in the mucigel, and also
within the tissues of the root (outer and inner cortex and stele).
The plant appears to benefit from the nitrogen fixed by the
bacteria; nodule formation does not occur (cf. ROOT NODULES).
There is some degree of host specificity: C4 plants (e.g. maize)
are infected by A. lipoferum, C3 plants (e.g. barley, oats, rice,
rye, wheat) by strains of A. brasilense.
Azotobacter A genus of Gram-negative, CYST-forming bacteria
(family AZOTOBACTERACEAE) which occur e.g. in fertile soils of
near-neutral pH. The cells are peritrichously flagellated or nonmotile, and are commonly short rods or coccobacilli though
A. paspali regularly forms both rods and long filaments; the
organisms appear to contain many copies of the chromosome
per cell [JGM (1984) 130 16031612]. Carbon sources used
by all species include e.g. glucose, fructose, sucrose, acetate,
fumarate, gluconate, and ethanol; most species can use nitrate
and/or ammonium salts as a source of nitrogen. In the presence
of combined nitrogen growth can occur within the pH range ca.
58.5; NITROGEN FIXATION occurs optimally within the pH range
77.5. In laboratory cultures nitrogen-fixing ability declines
with age, and is very poor immediately prior to encystment.
(Cyst-formation occurs maximally in old cultures on nitrogenfree media containing 0.2% butanol.) The optimum growth
temperature varies with species, and is ca. 3037 C. GC%: ca.
6368. Type species: A. chroococcum.
A. armeniacus. Peritrichously flagellated. Can use e.g. caprylate and mannitol but not e.g. caproate; some strains can use
propionate.
A. beijerinckii. Non-motile. Can use e.g. malonate and propionate but not caproate or rhamnose.
A. chroococcum. Peritrichously flaggellated. Can use e.g.
caproate, mannitol and propionate, but not e.g. caprylate.
A. nigricans. Non-motile. Cannot use caproate, propionate or
rhamnose. Some strains form e.g. a yellow or dark non-diffusible
pigment or a dark diffusible pigment.
A. paspali. Peritrichously flagellated. Cannot use caproate,
caprylate, malonate, mannitol, propionate or rhamnose, but can
use oxaloacetate, and some strains can use propan-1-ol. Appears
to occur only on (or within?) the root cortex of the grass
Paspalum notatum.
A. vinelandii. Peritrichously flagellated; non-motile strains
have been reported. Can use caproate, caprylate, malonate,
66
azygospore
drugs (e.g. PROBENECID) that inhibit glucuronidation may therefore affect the plasma concentration of AZT.
The use of AZT is associated with megaloblastic changes;
the drug may induce a dose-dependent macrocytic anaemia (less
often a severe normocytic anaemia) and is also able to induce
neutropenia [haematological aspects of HIV infection: BCH
(2000) 13 215230].
The value of AZT in anti-AIDS combination drug therapy
(against HIV-1) was indicated by an in vitro study in which
those nucleoside reverse transcriptase inhibitors which lacked
the 3 -azido moiety were less active against a particular mutant
form of the reverse transcriptase [AAC (2005) 49 11391144].
azthreonam Syn. AZTREONAM.
aztreonam (azthreonam) A MONOBACTAM derivative in which
R = an aminothiazoleoxime group, R = H, R = CH3 , R =
SO3 K+ (see b-LACTAM ANTIBIOTICS). It is active only against
aerobic Gram-negative bacteria, having a high degree of
specificity for PBP3 of Gram-negative bacteria (see PENICILLINBINDING PROTEINS); it is resistant to most b-lactamases. [Action,
use: Drugs (1986) 31 96130.]
Azuki bean mosaic virus See POTYVIRUSES.
azure See polychrome METHYLENE BLUE.
azurin (1) A BLUE PROTEIN which occurs in certain bacteria
(e.g. Alcaligenes denitrificans, Bordetella pertussis, Paracoccus
denitrificans, Pseudomonas aeruginosa); depending on source,
the MWt ranges from ca. 12000 to ca. 15000, and the Em appears
to be in the approximate range 230330 mV.
(2) A solution of CuSO4 and NH4 OH used as an agricultural
antifungal agent.
azygospore A parthenogenically derived spore, similar to a
ZYGOSPORE, formed e.g. by many species of the Mucorales.
mannitol, propionate and rhamnose. A yellowish-green watersoluble fluorescent pigment is formed on iron-deficient media.
[Book ref. 22, pp. 220229.]
Azotobacteraceae A family of Gram-negative (or Gramvariable), aerobic, chemoorganotrophic bacteria which occur
in soil, in the rhizosphere, and in aquatic habitats; the
organisms are capable of NITROGEN FIXATION typically under
free-living conditions, but sometimes in association with higher
plants. Cells: ovoid, or round-ended rods (sometimes filaments),
1.52.0 m or more in width, which may be motile (polarly
or peritrichously flagellated) or non-motile; some species form
cysts. Pigments, some fluorescent, are formed by some species.
PHB can be accumulated. Catalase +ve. Oxidase +ve (most
strains of most species). GC%: ca. 5268. Two genera:
AZOMONAS, AZOTOBACTER. [Book ref. 22, pp. 219234.]
azotoflavin See FLAVODOXINS.
AZT (3 -azido-3 -deoxythymidine; zidovudine) A thymidine
analogue ANTIRETROVIRAL AGENT used in the treatment of AIDS.
AZT is converted by cellular enzymes to the triphosphate derivative which is then incorporated instead of thymidine into
(provirus) DNA by the viral REVERSE TRANSCRIPTASE (see RETROVIRIDAE); the presence of the 3 -azido group inhibits further chain
elongation by preventing the formation of a phosphodiester bond
at the 3 position. Cellular DNA polymerase a is much less sensitive than reverse transcriptase to AZT triphosphate.
AZT competes for intracellular phosphorylation with another
NUCLEOSIDE REVERSE TRANSCRIPTASE INHIBITOR, stavudine.
As high-level resistance develops readily if AZT is used alone,
it is used in combination with other drugs.
Unlike other nucleoside reverse transcriptase inhibitors, AZT
undergoes significant metabolism (glucuronidation) in the liver;
67
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
B
No further development of the B cell occurs unless it
encounters specific antigen e.g. within so-called germinal centres
in the spleen or lymph nodes. In the event of contact with
specific antigen, the outcome depends e.g. on the type of
antigen involved and the contribution of T cells: see ANTIBODY
FORMATION. When a B cell is appropriately stimulated it prepares
for the role of antibody formation by initially undergoing BLAST
TRANSFORMATION and then proliferating to form a clone of cells
of identical antigenic specificity (= clonal expansion); some of
these cells develop as PLASMA CELLS while others (commonly)
become MEMORY CELLS.
B cells which do not bind specific antigen remain viable for
a limited period of time and subsequently undergo APOPTOSIS.
B-tubule (B-subfibre) See FLAGELLUM (b).
B-type inclusion body See POXVIRIDAE.
B-type particles See TYPE B ONCOVIRUS GROUP.
B-type starter See LACTIC ACID STARTERS.
B virus (cercopithecine herpesvirus 1; cercopithecid herpesvirus 1;
herpesvirus B; Herpesvirus simiae) A herpesvirus (subfamily
ALPHAHERPESVIRINAE) which naturally infects monkeys of the
genus Macaca. In rhesus monkeys (M. mulatta) infection may
be asymptomatic, or vesicular lesions (which may ulcerate)
may develop in the mouth and sometimes on the skin and
conjunctivae. B virus may be transmitted to humans e.g. by
monkey bites or scratches, and can cause in humans a severe
(usually fatal) encephalomyelitis (monkey-bite encephalomyelitis).
B12 coenzymes See VITAMIN B12 .
B19 parvovirus See ERYTHROVIRUS.
B663 CLOFAZIMINE.
BabesErnst granules METACHROMATIC GRANULES observed in
bacteria.
Babesia A genus of protozoa (subclass PIROPLASMASINA) parasitic in invertebrates and in the erythrocytes (RBCs) of vertebrates (cf. THEILERIA); at least some species (including B. equi
and B. microti ) develop in the lymphocytes (as well as in the
RBCs) of the vertebrate host, and it has been suggested that such
species be transferred to other genera (e.g. Nicollia, Nuttallia).
Some species (e.g. B. bigemina, B. bovis) can cause tick-borne
disease in domestic animals (see REDWATER FEVER), and some
(e.g. B. divergens, B. microti ) can cause disease in man [ARE
(1981) 26 9092]. The cells of Babesia are rounded or pyriform,
ca. 16 m. In the typical life cycle, sporozoites of Babesia are
injected into the vertebrate host by the tick vector, and each
sporozoite enters an RBC and undergoes schizogony to form two
or four merozoites which infect fresh RBCs when the host cell
ruptures. Following the ticks meal of infected blood, gametes
are formed in the ticks gut, and these fuse and give rise to a
(motile) kinete which passes, via various tissues, to the salivary
glands there undergoing sporogony and forming many sporozoites. Unlike Theileria, Babesia can invade the ovary and egg
of the tick, and can be transmitted transovarially to the ticks
offspring. [Life cycles of Babesia and Theileria: AP (1984) 23
37103.]
babesiosis Any disease of man or animals caused by a species
of BABESIA (e.g. REDWATER FEVER).
Bacillaria See DIATOMS.
Bacillariophyta See DIATOMS.
bacillary angiomatosis See BARTONELLA.
Bacillus
bacillary dysentery See DYSENTERY (a).
bacillary white diarrhoea Syn. PULLORUM DISEASE.
bacille CalmetteGuerin See BCG.
bacillin Syn. BACILYSIN.
bacillus (1) A member of the genus BACILLUS. (2) Any rodshaped bacterial cell, i.e., a cell whose length is ca. two or more
times greater than its width. (cf. COCCOBACILLUS and FILAMENT.)
A bacillus may be straight or curved (cf. VIBRIO sense 2), with
rounded, truncated or tapered ends (cf. FUSIFORM), and may occur
singly, in groups, pairs, chains, etc. (See also PALISADE.)
Bacillus
A genus of GRAM TYPE-positive, strictly aerobic or
facultatively anaerobic, typically catalase-positive, rod-shaped,
ENDOSPORE-forming bacteria. The organisms typically occur
as saprotrophs in soil and water, but certain species can be
pathogenic in man and other mammals (see e.g. B. anthracis
and B. cereus, below) and some species are entomopathogenic
(see e.g. B. moritai, B. popilliae and B. thuringiensis). [Insecticidal species: Book ref. 171, pp. 185209; MR (1986) 50
124.] Bacillus spp can cause biodeterioration (see e.g. FLAT
SOUR, LEATHER SPOILAGE, SWELL), but some species are used
commercially as sources of antibiotics (see e.g. BACITRACIN,
POLYMYXINS) or other products (e.g. DEBRANCHING ENZYMES, GLUCOSE ISOMERASE, GLYCEROKINASE, SUBTILISINS).
Cells: typically motile rods, commonly ca. 0.51.5
26 m, often in chains; some strains form a CAPSULE,
and some are pigmented. (See also S LAYER and TEICHOIC
ACIDS.) Metabolism may be respiratory (see RESPIRATION) some
strains being capable of NITRATE RESPIRATION or facultatively fermentative (see FERMENTATION); a few species (e.g.
B. macerans, B. polymyxa) can carry out NITROGEN FIXATION.
Most species are chemoorganoheterotrophs; B. schlegelii can
grow chemolithoautotrophically (see CARBOXYDOBACTERIA). Utilizable substrates for organoheterotrophic species range from
simple sugars and other carbohydrates to e.g. uric acid
(see B. fastidiosus) and proteinaceous materials; PENTOSES are
metabolized via the HEXOSE MONOPHOSPHATE PATHWAY. Many
species can grow on NUTRIENT AGAR. Storage compounds
include e.g. POLY-b-HYDROXYBUTYRATE. The genus includes psychrotrophs (e.g. B. globisporus), thermophiles (e.g. B. schlegelii,
B. stearothermophilus) and alkalophiles (e.g. B. alcalophilus,
B. firmus). GC%: ca. 3070. Type species: B. subtilis.
B. alcalophilus. An ALKALOPHILE (q.v.): optimum growth pH
ca. 910; no growth below pH 7.
B. alvei. See EUROPEAN FOULBROOD.
B. amyloliquefaciens. Similar or identical to B. subtilis. (See
also AMYLASES.)
B. amylolyticus. Nom. rev. [IJSB (1984) 34 224226].
B. aneurinolyticus. A species, related to B. brevis, which
produces a thiaminase. (See also BACTERIOPHAGE fBA1.)
B. anthracis. The causal agent of ANTHRAX. Cells: nonmotile, ca. 1.5 36 m, typically square-ended and usually
in chains. Virulent strains form a PLASMID-encoded toxin (see
ANTHRAX TOXIN) and a plasmid-encoded poly-D-glutamic acid
CAPSULE. [Capsule-encoding plasmid: see e.g. Inf. Immun.
(1985) 49 291297.] (cf. STERNE STRAIN.) Growth occurs on
nutrient agar. In biochemical tests B. anthracis gives results
very similar to those of B. cereus. Lecithinase activity is weak
or absent. Haemolysis on sheep-blood agar is weak or absent.
B. anthracis is susceptible to the g phage (B. cereus is not). On
agar containing benzylpenicillin (0.050.5 unit/ml) B. anthracis
gives rise to chains of enlarged, spherical cells (string of pearls
effect).
B. azotofixans. A proposed (nitrogen-fixing) species from
Brazilian soil [IJSB (1984) 34 451456].
bacillus CalmetteGuerin
and pectins, and most can carry out NITROGEN FIXATION. (See
also POLYMYXINS.)
B. popilliae. See MILKY DISEASE.
B. psychrophilus. A proposed (psychrophilic) species [IJSB
(1984) 34 121123].
B. pulvifaciens. Proposed species (isolated from a diseased
bee) [IJSB (1984) 34 410413].
B. pumilus. Cells: typically slender (0.51.0 m wide); usually motile. Spore: elongated, not distending the cell. Metabolically similar to B. subtilis, but starch is not utilized. Usually VP
+ve.
B. schlegelii. See CARBOXYDOBACTERIA and HYDROGEN-OXIDIZING BACTERIA.
B. sphaericus. Cells: slender (ca. 0.51.0 m wide); usually
motile. Spore: spherical, distending the cell. Typically, carbohydrates are not utilized. Can cause LEATHER SPOILAGE, and can be
insecticidal to e.g. mosquito larvae toxicity apparently being
due to an uncharacterized toxin and not associated with sporulation. [Field evaluation of a B. sphaericus strain as a mosquito
biocide: J. Inv. Path. (1986) 48 133138.]
B. stearothermophilus. Thermophilic; can grow at e.g. 65 C.
Cells: ca. 1.0 m wide; spore: ellipsoidal, often distending the
cell. The spores are highly resistant to heat, and are sometimes
used to monitor AUTOCLAVE performance. (See also FLAT SOUR.)
Typically, a range of carbohydrates can be metabolized anaerobically and anaerogenically; the main product of carbohydrate
fermentation commonly appears to be lactic acid. (See also GLYCEROKINASE.)
B. subtilis. Cells: slender (typically ca. 0.8 m wide), usually motile; chains are uncommon. (See also CERULENIN and
MACROFIBRE.) Spore: ellipsoidal, usually not distending the cell.
Metabolism appears to be primarily respiratory. Growth does not
occur in anaerobic glucose broth. Glucose, various other sugars
and sugar alcohols, and starch, are metabolized anaerogenically.
VP +ve. Nitrate is reduced. Casein and gelatin are hydrolysed.
Phages which infect B. subtilis include e.g. BACTERIOPHAGE PBS1,
BACTERIOPHAGE f105 and BACTERIOPHAGE SPO1.
B. thuringiensis. An entomopathogenic species which is morphologically and biochemically very similar to B. cereus, differing primarily in its formation of DELTA ENDOTOXIN (q.v.).
B. validus. Nom. rev. [IJSB (1984) 34 224226].
Other species include e.g. B. insolitus, B. laterosporus,
B. lentus, and B. pantothenticus.
Note on the identification of species. Some mutually contradictory tables of biochemical test reactions have been published.
For example, the VP test reactions (obtained using traditional
methods) given in Book ref. 46, p. 1731 differ significantly, in
respect of a number of species, from those (obtained using the
API system) given in JGM (1984) 130 18711882. (Species
designated as VP +ve above are confirmed as such in many
sources.)
bacillus CalmetteGuerin See BCG.
bacilysin (bacillin; tetaine) A dipeptide ANTIBIOTIC which is
active against a wide range of Gram-positive and Gramnegative bacteria and e.g. against Candida albicans. It consists
of a C-terminal epoxy-L-amino acid (anticapsin) and an Nterminal L-alanine residue; it is taken up by peptide transport
systems in sensitive cells, and is subsequently hydrolysed by
cellular enzymes to release the anticapsin an inhibitor of
glucosamine (and hence e.g. PEPTIDOGLYCAN) synthesis. (cf.
WARHEAD DELIVERY.)
bacitracin A cyclic dodecapeptide ANTIBIOTIC produced by
strains of Bacillus spp. It is active against many Grampositive and certain Gram-negative bacteria (e.g. Neisseria spp,
Haemophilus spp). In the presence of divalent cations (particularly Zn2+ ) bacitracin binds to bactoprenol pyrophosphate,
inhibiting the regeneration of bactoprenol monophosphate during e.g. PEPTIDOGLYCAN biosynthesis; it can also inhibit other
processes involving bactoprenol pyrophosphate (e.g. O-specific
chain formation in LIPOPOLYSACCHARIDE biosynthesis) and can
affect membrane permeability. Bacitracin is used clinically e.g.
for the topical treatment of local infections, and as a FEED ADDITIVE for ruminants to decrease methane production in the RUMEN.
back focal plane Of a convex lens: the focal plane furthest from
the light source.
back mutation (reverse mutation) (1) A MUTATION which reverses the effects of a FORWARD MUTATION by restoring the original
nucleotide sequence. (2) Either a mutation as in sense 1 above,
or an intragenic SUPPRESSOR MUTATION.
background mutation Syn. SPONTANEOUS MUTATION.
bacon spoilage See MEAT SPOILAGE.
BACTEC culture systems Liquid media (marketed by Becton Dickinson) which can be used e.g. for the growth of
Mycobacterium tuberculosis growth being detectable more
rapidly (12 weeks) than is usually possible on solid
media (6 weeks). These media may be used for (i) detecting
M. tuberculosis in clinical specimens, and (ii) examining an isolate of the pathogen for susceptibility to antibiotics; for the latter
purpose an isolate is tested for growth (or lack of growth) in a
medium containing a known amount of the given antibiotic.
Earlier BACTEC systems were radiometric, i.e. they detected
growth by detecting radioactive carbon dioxide produced from a
radioactive substrate in the medium. A more recent system, the
BACTEC MGIT 960 (MGIT = mycobacteria growth indicator
tube), monitors growth by means of a fluorescent sensor
system which detects the consumption of oxygen. [Evaluation
of BACTEC MGIT 960: JCM (1999) 37 748752.]
bacteraemia (bacteremia) The condition in which viable bacteria
are present in the bloodstream. (cf. PYAEMIA; SEPTICAEMIA.)
bacteremia Syn. BACTERAEMIA.
bacteria (singular: bacterium) (1) Formerly: a term which
referred, collectively, to all prokaryotic microorganisms (see
PROKARYOTE); the term was also used to refer to a population
of specific prokaryote(s) of any given type.
(2) All, or particular, members of the domain Bacteria (see
next entry).
Note. In literature prior to the 1980s bacteria was always
used with the meaning given in sense 1. With the establishment
of the domain ARCHAEA (q.v.), appropriate usage is that given in
sense 2.
Bacteria A taxon (DOMAIN) comprising one of the two fundamentally distinct groups of prokaryotic microorganisms (see
PROKARYOTE and ARCHAEA). (See also previous entry.)
The bacteria are a diverse group of (usually) single-celled
organisms. Most are free-living, occurring e.g. in soil, on plants,
in various aquatic habitats, and even in antarctic snow [AEM
(2000) 66 45144517]; some are important in the cycles of
matter (see CARBON CYCLE, NITROGEN CYCLE, SULPHUR CYCLE).
Bacteria are also found as symbionts in plants, animals and
certain microorganisms (see CAEDIBACTER, MYCETOCYTE, ROOT
NODULES, RUMEN).
A minority of bacteria occur as intracellular or extracellular parasites or pathogens in man and/or other animals.
In man, bacteria can cause a number of major and minor
diseases which include e.g. ANTHRAX, BOTULISM, BRUCELLOSIS, CHOLERA, DIPHTHERIA, DYSENTERY, ERYSIPELAS, GONORRHOEA, LEGIONNAIRES DISEASE, LEPROSY, LYME DISEASE, MENINGITIS, PLAGUE, PSEUDOMEMBRANOUS COLITIS, Q FEVER, SCARLET
70
Bacteria
Bacteria
Archaea
CYANOBACTERIA
GRAM POSITIVE
EURYARCHAEOTA
Anabaena sp
Bacillus subtilis
Clostridium perfringens
Corynebacterium xerosis
Enterococcus faecalis
Lactobacillus delbrueckii
Listeria monocytogenes
Mycobacterium tuberculosis
Propionibacterium acnes
Streptomyces coelicolor
Halobacterium halobium
Desulfurococcus mobilis
Methanobacterium bryantii
Methanococcus jannaschii
Pyrodictium occultum
Gloeobacter sp
Oscillatoria sp
Prochloron didemni
Thermoplasma acidophilum
CRENARCHAEOTA
Sulfolobus solfatarius
Thermoproteus tenax
PROTEOBACTERIA
(Alpha)
(Beta)
(Gamma)
(Epsilon)
Agrobacterium tumefasciens
Alcaligenes faecalis
Coxiella burnetii
Helicobacter pylori
Brucella abortus
Bordetella pertussis
Escherichia coli
Rickettsia spp
Neisseria gonorrhoeae
Neisseria meningitidis
Haemophilus influenzae
Legionella pneumophila
Spirillum natans
Proteus vulgaris
Pseudomonas aeruginosa
Vibrio parahaemolyticus
BACTERIA: examples of species in some of the groups in a current taxonomic scheme for the Bacteria (some species of the domain Archaea
are also shown); the lines are not intended to reflect evolutionary distances between the organisms. A number of groups not shown in the
figure are outlined in the text; note, for example, that the Gram-positive species are divided into high GC% and low GC%.
Reproduced from Bacteria, 5th edition, Figure 16.5, page 436, Paul Singleton (1999) copyright John Wiley & Sons Ltd (UK) (ISBN
0471-98880-4) with permission from the publisher.
FEVER, SYPHILIS, TETANUS, TOXIC SHOCK SYNDROME, TRACHOMA,
71
bacteriocin
studies on pediocin PA-1 (a class IIa bacteriocin produced by
Pediococcus spp) reported binding to lipsomes in the absence
of a protein receptor [AEM (1997) 63 524531] suggesting
that a protein receptor may not be an absolute requirement for
these bacteriocins; it may be that these (cationic) bacteriocins
bind to anionic phospholipid groups in the membrane.
A given bacteriocin acts on a susceptible target cell in a
characteristic way. Some bacteriocins (e.g. some colicins, lantibiotics) form pores in the cytoplasmic membrane; some (e.g.
microcin B17) inhibit DNA gyrase; some (e.g. LYSOSTAPHIN)
disrupt PEPTIDOGLYCAN; and some (e.g. CLOACIN DF13) cleave
16S rRNA. It appears that, in some cases, a single bacteriocin
molecule can be lethal for a sensitive cell. (Although bacteriocins are active primarily against bacteria, certain colicins and
VIBRIOCINS have been reported to affect some types of eukaryotic
cell [JAC (1980) 6 424427].)
Various mechanisms provide a cell with immunity to the bacteriocin(s) it encodes. For example, while cells actively secreting
colicins are damaged by their lysis proteins, neighbouring cells
of the same strain, repressed for colicin synthesis, are protected by immunity proteins (see COLICINS). Cells producing
LYSOSTAPHIN achieve immunity by modifying their own peptidoglycan. Cells producing the lantibiotic EPIDERMIN achieve
immunity by operating an ATP-dependent pump (transport system) which actively secretes any molecules of the agent that are
taken up.
Biotechnological applications of bacteriocins. The great diversity of bacteriocins, and the ability of many of them to kill/inhibit
certain pathogenic bacteria, has prompted much research into the
possibility of using particular bacteriocins as antibiotics and/or
as food preservatives/additives (see e.g. LACTICIN 3147).
Particularly useful bacteriocins are produced by certain LACTIC ACID BACTERIA (e.g. species of Carnobacterium, Enterococcus, Lactobacillus and Lactococcus), some of which are highly
active against important food-borne pathogens (such as Listeria
monocytogenes). According to structural and other characteristics, bacteriocins of the lactic acid bacteria have been classified
into four classes [FEMS Reviews (1993) 12 3986]:
Class I. LANTIBIOTICS: small, typically pore-forming peptides
containing unusual constituents (such as lanthionine) e.g.
EPIDERMIN and NISIN.
Class II. Small peptides (<10 kDa) which lack unusual constituents (such as lanthionine) and which have a specific form
of processing site in the precursor molecule; they exhibit stability at e.g. 100120 C. This category is divided into three
subgroups. Class IIa bacteriocins contain a specific N-terminal
sequence, and all are highly active against Listeria spp. They
include PEDIOCIN PA-1 and SAKACIN A. [Biosynthesis, structure
and activity of class IIa bacteriocins: FEMS Reviews (2000)
24 85106.] Class IIb bacteriocins are two-component, poreforming agents. They include e.g. lactacin F and lactococcin G.
Class IIc bacteriocins are thiol-activated peptides which require
reduced cysteine residues for activity.
Class III. Large (>30 kDa) heat-labile proteins; they include
helveticin J, lactacin A and lactacin B.
Class IV. Bacteriocins which consist of a protein moiety
plus at least one non-protein (e.g. lipid) constituent which is
necessary for activity. They include lactocin 27, leuconocin S
and plantaricin S.
Other bacteriocins. See also PESTICIN I, PYOCINS, STAPHYLOCOCCIN and ULCERACIN 378. Bacteriocins are also produced by
Bacillus megaterium (megacins), Klebsiella spp (klebicins), Listeria monocytogenes (monocins [Zbl. Bakt. Hyg. A (1986) 261
Gram-positive and Gram-negative bacteria, which are bacteriostatic or bactericidal often specifically to organisms that are
closely related to the bacteriocin-producing strain. Bacteriocins
include e.g. COLICINS, MICROCINS and LANTIBIOTICS.
Agents analogous to bacteriocins are produced by members
of the Archaea; these agents (e.g. the halocins produced by
halobacteria) are apparently not homologous to any bacteriocin
in terms of amino acid sequences.
In size and structure, bacteriocins range from a simple modified amino acid (microcin A15), through short peptides and
high-MWt colicins, to phage-like PYOCINS. (See also BACTERIOPHAGE fBA1.) Some bacteriocins (lantibiotics) undergo distinctive post-translational modification which is necessary for their
activity. The lantibiotic LACTICIN 3147 (produced by Lactobacillus lactis subsp lactis) is a two-component bacteriocin both
peptides being necessary for activity; moreover, each of the two
peptides needs modification by a separate enzyme [Microbiology
(2000) 146 21472154].
Evolutionary relationships are evident within some groups of
bacteriocins. [Molecular mechanisms of bacteriocin evolution:
ARG (1998) 32 255278.]
Bacteriocins are commonly encoded by PLASMIDS (see e.g.
COLICIN PLASMID); bacteriocin-encoding plasmids include both
conjugative and non-conjugative types. Examples of chromosomally encoded bacteriocins include bacteriocin 28b (a colicin
encoded by Serratia marcescens) and some of the class IIa bacteriocins produced by lactic acid bacteria (see later).
The mode of regulation of bacteriocin synthesis varies among
the different groups. For example, synthesis of colicins is promoted by those conditions which trigger the SOS SYSTEM (see
COLICIN PLASMID). By contrast, many bacteriocins of the lactic
acid bacteria appear to be regulated by a three-component system
which includes a histidine protein kinase, a response regulator,
and an induction factor. (cf. TWO-COMPONENT REGULATORY SYSTEM). Induction factors (IFs) are small heat-stable peptides produced by the bacteriocinogenic cell. The mechanism by which
IFs promote synthesis of bacteriocin is unknown, but it has been
suggested that they may trigger synthesis as a result of their gradual intracellular accumulation or that their influence may reflect
environmental factors. Synthesis of the bacteriocin sakacin A
(produced by Lactobacillus sake) is reported to be regulated
by a three-component system (which includes a 23-amino-acid
cationic peptide) in a temperature-sensitive way [Microbiology
(2000) 146 21552160]. The bacteriocin divercin V41, produced
by Carnobacterium divergens strain V41, may be regulated by a
two-component system [Microbiology (1998) 144 28372844].
The different types of bacteriocin are released in different ways from the cells which synthesize them. For example,
release of colicins depends on a lysis protein which causes
a (non-specific) increase in the permeability of the cell envelope allowing dispersal of the bacteriocin (but with concomitant adverse effects on the producing cell). By contrast, certain
bacteriocins (e.g. ENTEROCIN P) are secreted via a sec-dependent
pathway, while some class IIa bacteriocins of the lactic acid
bacteria are reported to be secreted by ABC TRANSPORTERS.
The import of some types of bacteriocin (e.g. colicins) into
sensitive cells depends on the binding of the bacteriocin to a specific cell-surface receptor. In most or all cases, uptake of colicins
appears to be an energy-dependent process (pmf being needed
for transport across the outer membrane, and ATP hydrolysis
being involved in transport across the cytoplasmic membrane);
the route of translocation through the cell envelope depends on
the given colicin (see groups A and B COLICINS). By contrast,
73
bacteriocin 28b
bacteriocyte In certain invertebrates, particularly insects: a specialized cell which contains intracellular bacterial symbionts.
(cf. MYCETOCYTE.) Bacteriocytes occur e.g. in the cockroach
(see BLATTABACTERIUM), in some marine sponges (containing
Aphanocapsa endosymbionts) and in aphids (see BUCHNERA).
bacteriolysis The lysis (rupture) of bacterial cells. In nature,
various microorganisms produce enzymes or antibiotics which
lyse bacteria either to provide nutrients or (presumably)
for competitive advantage. (See e.g. ANAEROPLASMA, ENSIFER,
LYSOSTAPHIN, MUSHROOM CULTIVATION, MYXOBACTERALES.) Most
BACTERIOPHAGES eventually lyse their host cells to release their
progeny. In the laboratory bacteria may be lysed mechanically
or enzymically (see CELL DISRUPTION).
bacterio-opsin See OPSIN.
bacteriophaeophytin A PHAEOPHYTIN derivative of a bacteriochlorophyll. Bacteriophaeophytins occur e.g. in the REACTION
CENTRES in a number of purple photosynthetic bacteria and
in the cytoplasmic membrane of some green photosynthetic
bacteria.
bacteriophage (phage) Any VIRUS whose host is a bacterium.
(Viruses which infect cyanobacteria are conventionally called
CYANOPHAGES.) Most probably all bacteria can be infected
by particular phages; commonly, a given phage can infect only
one or a few strains or species of bacteria. The consequences of
phage infection depend on phage and host, and to some extent on
Virion morphology
Principal host(s)
Escherichia coli
enterobacteria
Acholeplasma laidlawii
Escherichia coli
Escherichia coli
Escherichia coli
Salmonella
Bacillus subtilis
Bacillus subtilis
Escherichia coli
enterobacteria
various
Acholeplasma laidlawii
filamentous or rod-shaped
icosahedral
various
enterobacteria
Genome: dsRNAb
f6
enveloped nucleocapsid
icosahedral
various
dsDNAb
Genome: linear
l
Mu
MV-L3
N4
P1
P2
P22
f29
SPO1
T4
T7
Tectiviridae (e.g. PRD1, AP50)
Genome: ccc dsDNAb
MV-L2
PM2
Alteromonas espejiana
ssRNAb
Genome:
Leviviridae (e.g. MS2, Qb)
a
b
bacteriophage conversion
have indicated that, on attaching to the host cell, the phage ejects
proteins that may assemble to form a channel across the bacterial
cell envelope through which the genome is translocated; it has
been speculated that two of the ejected proteins may form the
components of a motor that rachets phage DNA into the host
cell [Mol. Microbiol. (2001) 40 18].
For phage development to proceed, the phage nucleic acid
must escape degradation by the hosts RESTRICTION ENDONUCLEASE system. For a general account of viral replication strategies
see VIRUS; for detailed accounts of particular phages see following entries. Virion assembly may occur by the spontaneous
aggregation of the various phage components, but the more complex virions require the participation of non-structural phagecoded proteins (see SCAFFOLDING PROTEIN). Host cell lysis may
be induced by phage-coded enzymes or by activation of host
cell autolysins. (See also LYSIS FROM WITHOUT, LYSIS PROTEIN and
ONE-STEP GROWTH EXPERIMENT.)
Bacteriophages can cause considerable economic problems
in certain biotechnological processes such as the manufacture
of dairy products, antibiotics, etc. A few phages are medically
important in that they encode certain toxins (see BACTERIOPHAGE
CONVERSION). In microbiology, phages are useful e.g. for PHAGE
TYPING, for achieving gene transfer between bacteria (see TRANSDUCTION), for probing the molecular biology of bacteria, etc.
Phages may be cultivated and/or assayed e.g. by inoculation
at low multiplicity of infection on a LAWN PLATE of susceptible
bacteria (see PLAQUE and PLAQUE ASSAY). They may also be
cultivated in broth cultures of host bacteria, the activity of
virulent phages being indicated by the progressive decrease in
turbidity of the culture as the cells lyse; a suspension of phages
may be prepared from the lysate e.g. by CENTRIFUGATION or by
membrane FILTRATION to remove bacterial debris.
bacteriophage 7-7-1 See FLAGELLOTROPIC PHAGE.
bacteriophage 21 See LAMBDOID PHAGES.
bacteriophage 82 See LAMBDOID PHAGES.
bacteriophage 434 See LAMBDOID PHAGES.
bacteriophage 1307 See PLASMAVIRIDAE.
bacteriophage a3 See MICROVIRIDAE and BACTERIOPHAGE G4.
(Also: a dsDNA-containing phage of Achromobacter sp 2
[JGV (1981) 53 275281].)
bacteriophage a15 See LEVIVIRIDAE.
bacteriophage AP50 See TECTIVIRIDAE.
bacteriophage Bam35 See TECTIVIRIDAE.
bacteriophage b See LEVIVIRIDAE. (cf. Corynephage b see
DIPHTHERIA TOXIN.)
bacteriophage BF23 A bacteriophage which infects Escherichia
coli and which resembles phage T5. (See also BTUB PROTEIN.)
bacteriophage BPB1 See STYLOVIRIDAE.
bacteriophage Cf See INOVIRUS.
bacteriophage c See STYLOVIRIDAE.
bacteriophage conversion (phage conversion) In a bacterium:
the acquisition, loss or modification of one or more phenotypic characteristics as a result of infection by a BACTERIOPHAGE typically a temperate phage (lysogenic conversion); it
may result e.g. from the expression of phage genes or from
inactivation of one or more bacterial genes due to insertion of a
prophage into the bacterial chromosome. (Phenotypic alteration
in a recipient cell due to TRANSDUCTION of bacterial DNA is not
regarded as phage conversion.)
Phage conversion is responsible for toxigenicity in a number
of pathogenic bacteria. For example, phages encode CHOLERA
TOXIN, DIPHTHERIA TOXIN and the shiga-like toxins of enterohaemorrhagic strains of Escherichia coli (including O157:H7)
bacteriophage CTX8
bacteriophage fr See LEVIVIRIDAE.
bacteriophage G4 An isometric SSDNA PHAGE of the MICROVIRIDAE. On penetrating the host cell, the ss cccDNA genome is
coated with host SSB protein; a GC-rich region between genes F
and G probably remains uncoated. Stage I (see SSDNA PHAGE) is
independent of host dnaB function (as it is in microviruses St-1,
a3, fK and fXtB cf. BACTERIOPHAGE fX174). The F G intergenic region seems to fold into a secondary structure [JV (1986)
58 450458] which is capable of direct (dnaB-independent)
recognition by host PRIMASE (cf. PRIMOSOME and DNAB GENE).
Primase synthesizes a short RNA primer at a unique site (ori )
in the intergenic region. The c strand is completed as in other
SSDNA PHAGES. Stage II in G4 requires dnaB function, presumably for initiation of n strand synthesis. (Phages St-1, fK and
a3 do not require dnaB at any stage.) G4 n strand synthesis
begins at the n strand origin (Ov ) in gene A; the c strand origin
(Oc ) in the F G intergenic region is on the opposite side of the
molecule. n strand synthesis seems to proceed by the displacement of the old n strand as a closed loop (D LOOP) at the Ov
site, and hence is independent of a gpA-induced nick (cf. BACTERIOPHAGE fX174). Synthesis of n strand by DNA polymerase
III holoenzyme and Rep protein proceeds unidirectionally. When
the replication fork passes Oc , primer synthesis can begin on the
displaced loop, and c strand synthesis can proceed in the opposite direction. The parental n and c circles may separate before
replication of either is complete. G4 seems to resemble fX174
(q.v.) in stage III and morphogenesis.
bacteriophage G6 See MICROVIRIDAE and BACTERIOPHAGE fX174.
bacteriophage G13 See MICROVIRIDAE and BACTERIOPHAGE fX174.
bacteriophage G14 See MICROVIRIDAE and BACTERIOPHAGE fX174.
bacteriophage HM3 See MYOVIRIDAE.
bacteriophage I3 See MYCOBACTERIOPHAGES.
bacteriophage If1 An INOVIRUS which adsorbs specifically to
I-type pili of enterobacterial hosts; phage If2 is very similar.
bacteriophage If2 See BACTERIOPHAGE IF1.
bacteriophage IKe An INOVIRUS specific for enterobacteria
which contain an IncN plasmid; the phage can apparently establish a pseudolysogenic infection of its host [CJM (1978) 24
15951601]. [Nucleotide sequence and genetic organization of
IKe genome: JMB (1985) 181 2739.]
bacteriophage L1 group See PLECTROVIRUS.
bacteriophage L2 group See PLASMAVIRIDAE.
bacteriophage L3 group See MV-L3 PHAGE GROUP.
bacteriophage L4 A BACTERIOPHAGE closely related to BACTERIOPHAGE P22 but defective in maintenance of lysogeny; it is commonly used as a transduction vector in Salmonella typhimurium.
bacteriophage L17 See TECTIVIRIDAE.
bacteriophage L34a See BACTERIOPHAGE CONVERSION.
bacteriophage l A temperate BACTERIOPHAGE (family STYLOVIRIDAE) which infects Escherichia coli. Head: icosahedral, ca.
55 nm diam., composed of two major structural proteins (gpE
and gpD) and several minor proteins (gpB, gpC, gpFII ). Tail:
long (ca. 150 10 nm), flexible, tubular, non-contractile, joined
to the head via a neck or connector region, and terminating
at the distal end in a small basal structure to which is attached a
single fibre (the adsorption organelle). (See also LAMB PROTEIN.)
Genome: linear dsDNA (48514 bp long [nucleotide sequence:
JMB (1982) 162 729773]) with single-stranded 12-base 5
STICKY ENDS (designated cos). On infection of a host cell, phage
DNA is transferred to the host through the tail and is immediately
circularized by base-pairing between the sticky ends followed by
host DNA ligase action. Subsequent events may eventually lead
either to host cell lysis (involving the production and release of
bacteriophage l
head and tail genes
and morphogenesis
cos A
att
recombination
int xis
red
DNA
replication
regulation
gam cIII
pI
N
pL
cI
cro
pR
cII
pRE
lysis
Q
ori
R cos
pR
pRM
Nu3
Nu1AWB C D E F I F II Z U V G T HM L K I J
cIII
nutL cI
oL
pL
BACTERIOPHAGE l. Simplified map of the virion genome (not drawn to scale). See entry for explanation.
bacteriophage M12
events of the lytic cycle. In contrast to pL -initiated transcription
in the lytic cycle, pL -initiated transcription in the prophage
results in the expression of both int and xis (necessary for
excision). This is possible because, owing to the permuted gene
order in the prophage, the sib-containing b region is no longer
immediately downstream from int; the pL -initiated transcript is
thus not recognized by RNase III, and both int and xis can be
expressed.
[General review: Book ref. 79; lhost interactions: MR
(1984) 48 299325.]
bacteriophage M12 See LEVIVIRIDAE.
bacteriophage M13 See INOVIRUS.
bacteriophage MS2 See LEVIVIRIDAE.
bacteriophage Mu A temperate bacteriophage which can infect
various enterobacteria (e.g. Escherichia coli, Citrobacter freundii, Erwinia spp, and certain mutant strains of Salmonella
typhimurium). The phage particle has an icosahedral head (ca.
60 nm diam.) and a contractile tail (ca. 100 nm long when
extended, 60 nm when contracted) to which is attached a base
plate with spikes and tail fibres; the phage tail adsorbs to LPS in
the outer membrane of a host cell. Phage particles contain linear
dsDNA ca. 39 kb long.
An early event after phage infection regardless of whether
infection will eventually result in a lytic cycle or the lysogenic
state is the integration of Mu DNA into the host chromosome
at a more or less randomly selected location. Integration often
results in the inactivation of the gene in which it occurs;
ca. 23% of bacteria in a population acquire a recognizable
mutation on lysogenization by Mu, a frequency much greater
than the spontaneous mutation rate in the absence of Mu i.e.,
Mu acts as a mutator phage (Mu = abbr. for mutator). The initial
integration event may be conservative (i.e., both strands of the
Mu DNA may be inserted) and appears to be a simple (nonreplicative) insertion; it requires the product of Mu gene A which
can recognize and bind to the ends of Mu DNA [Cell (1984) 39
387394]. Synthesis of a repressor (the c gene product) results
in lysogeny and immunity to superinfection by Mu.
During the lytic cycle, Mu DNA replication occurs entirely
by repeated replicative transposition of the integrated DNA
(which thus functions as a giant TRANSPOSON, causing chromosomal deletions, inversions, duplications etc); Mu DNA insertion
results in a 5-bp duplication of the target DNA (cf. Tn3 ). Transposition occurs at very high frequency (ca. 100 transpositions
per cell in ca. 30 min), copies of Mu DNA being inserted at
random locations in the chromosome; this results in the death
of the host cell, and ca. 100 progeny phages are released ca.
60 min after infection. Transposition is controlled by the products of phage genes A and B and requires continual synthesis of
gpA which apparently acts stoichiometrically; gpA functions
as a transposase, gpB apparently functions in the modification
of gpA activity. [Role of DNA topology in Mu transposition:
Cell (1986) 45 793800.]
Phage Mu DNA contains three regions, designated a (ca.
33 kb), G (ca. 3 kb) and b (ca. 1.7 kb), flanked by random
sequences of bacterial DNA (see below). The a region contains
most of the phage genes, including e.g. the repressor (c)
gene, all the early functions, all the head functions, and most
of the tail functions. The G region carries the remainder of
the tail functions and specifies the host range of the phage.
The G segment is flanked by short inverted repeats, and can
invert by reciprocal recombination between these sequences;
when in one orientation, designated G(+), it specifies a host
range which includes E. coli K12 strains, but in the alternative
bacteriophage P1
bacteriophage MV-L51 See PLECTROVIRUS.
bacteriophage 06N 58P See CORTICOVIRIDAE.
bacteriophage N4 A virulent coliphage of the PODOVIRIDAE.
Genome: linear dsDNA (ca. 71 kb) containing terminal direct
repeats 400450 bp long and a 7-base 3 overhang at one
end. The phage particle contains a rifampicin-resistant DNAdependent RNA polymerase which is injected into the host
cell with the DNA and which is necessary for transcription of
N4 early genes. Transcription of intermediate (middle) genes
requires the synthesis and activity of three N4 early proteins,
two of which are components of a second rifampicin-resistant
RNA polymerase; transcription of late genes requires E. coli
RNA polymerase activity. Host DNA replication is blocked by
an N4 early gene product, but host RNA and protein synthesis
continues (except in the case of cAMP-dependent operons). The
N4 genome codes for most functions required for its replication,
including a DNA polymerase and DNA-binding protein; the
only host functions it appears to require are gyrase, DNA
polymerase 5 3 exonuclease activity, DNA ligase, and nrdA
gene function [Book ref. 69, pp. 245254].
bacteriophage P1 A temperate BACTERIOPHAGE (family MYOVIRIDAE) which infects Escherichia coli and Shigella spp. Virion:
icosahedral head (ca. 90 nm diam.) with a long, complex contractile tail bearing a base-plate and tail fibres. Genome: dsDNA
(MWt ca. 66 106 ), circularly permuted and terminally redundant. On infection of a host cell, the genome circularizes (with
loss of redundancy) and may enter a LYTIC CYCLE or establish
LYSOGENY. Relatively little is known about the lytic cycle; both
q- and s-type modes of DNA replication occur early in infection,
but later only s-type replication can be observed. DNA packaging occurs by a headful mechanism, starting at a unique site
(pac); cleavage of DNA at a pac site apparently occurs early
in infection, before phage heads are formed, and the enzyme
responsible may remain bound to the DNA and subsequently
interact with a prohead to initiate packaging. (cf. BACTERIOPHAGE P22.)
In the lysogenic state, the P1 prophage does not normally integrate into the host chromosome, but persists as an autonomous,
circular PLASMID (P1 plasmid) which is maintained at one or two
copies per host chromosome. The replication control system of
the P1 plasmid resembles that of the F PLASMID (q.v.) e.g. in that
it involves a plasmid-encoded protein (designated RepA in the
P1 plasmid) which is essential for replication and which autoregulates its own synthesis. Moreover, the repA gene is flanked on
each side by multiple 19-bp repeat sequences, and it appears
that one of these multiple repeats (incA) may be involved in the
control of copy number in that it appears to titrate the RepA
protein. [P1 replication: JBC (1986) 261 35483555.] The P1
plasmids are segregated (see PARTITION) with great accuracy at
each host cell division, and spontaneous loss of the plasmid is
extremely rare. This high degree of accuracy involves several
mechanisms. For example, P1 encodes a SITE-SPECIFIC RECOMBINATION (SSR) system which facilitates accurate partition by
efficiently resolving plasmid dimers into monomers. (Dimers are
formed by homologous recombination between the two plasmids
resulting from replication.) This system involves a site (loxP ) on
the plasmid at which SSR occurs, and a gene (cre) encoding the
recombinase. (The lox-Cre system also catalyses cyclization of
the phage genome on infection of the host at least in RecA
hosts; it can also mediate the rare integration of the P1 plasmid
into the host chromosome at a site designated loxB.) [Regulation of the cre gene: JMB (1986) 187 197212.] Partition
per se involves a sequence (par ) in the plasmid; a gene (parA)
bacteriophage P2
consists of an icosahedral head (ca. 60 nm diam.) attached via
a short tubular neck to a tail which is essentially no more
than a hexagonal base-plate bearing short spikes. The tail
region has endorhamnosidase activity. Genome: dsDNA (MWt
ca. 26 106 ), terminally redundant, and circularly permuted in
certain regions of the genome.
On infection of a host cell, the linear DNA is circularized
either by the host RecA system or by a general recombinase
encoded by the P22 erf gene. In the lytic cycle, the DNA may
undergo some replication in the circular form; subsequently, concatemers many unit genomes in length are produced. During
virion assembly, a prohead consisting mainly of coat protein
(gp5) and a SCAFFOLDING PROTEIN (gp8) interacts with a concatemeric DNA molecule; DNA is encapsidated, beginning at a
specific site (pac) in the concatemer and proceeding sequentially
until the head is full, and the scaffolding protein is eliminated
intact (and is recycled). It appears that once the first packaging
event has been completed, the remaining DNA of the concatemer
is encapsidated by other proheads i.e., the leading end of the
DNA which enters the second and subsequent proheads is determined not by the pac site but by the length of DNA packaged
by previous prohead(s). (The mechanism of this is uncertain;
the initial cleavage at the pac site can apparently occur in the
absence of encapsidation [JMB (1982) 154 565579].) (cf. BACTERIOPHAGE P1.) Maturation of the virion requires the addition of
certain minor phage proteins. (See also TRANSDUCTION.)
The lysogenic pathway in P22 is essentially similar to that in l
(see LAMBDOID PHAGES). The prophage inserts in the Salmonella
chromosome at a site between proA and proC ; insertion is
catalysed by a P22-specified integrase encoded by an int gene
located close to the att site.
bacteriophage PA2 See STYLOVIRIDAE.
bacteriophage PBS1 A large, morphologically complex FLAGELLOTROPIC PHAGE (family MYOVIRIDAE) which infects Bacillus
subtilis; its DNA contains deoxyuridine instead of thymidine.
PBS1 is a pseudotemperate phage, establishing a carrier state in
its host (see PSEUDOLYSOGENY); it can mediate transduction.
bacteriophage PBSX A defective bacteriophage, the prophage of
which is normally present in the chromosome of its host, Bacillus
subtilis. When induced by mitomycin C, PBSX packages 13-kb
lengths of DNA which may include sequences from any region
of the host chromosome, packaging probably occurring by a
headful mechanism [JV (1985) 54 773780].
bacteriophage Pf1 See INOVIRUS.
bacteriophage Pf2 See INOVIRUS.
bacteriophage fI See T7 PHAGE GROUP.
bacteriophage fII See T7 PHAGE GROUP.
bacteriophage f6 The sole member of the family Cystoviridae.
Host: Pseudomonas syringae pv. phaseolicola; plaques clear,
diam. 13 mm. Some strains of P. pseudoalcaligenes can be
infected. The virion (diam. ca. 75 nm) has a segmented genome
of three pieces of dsRNA designated L, M and S (MWt ca. 5.0,
3.1 and 2.3 106 , respectively). [Nucleotide sequence of, and
translational control in, the S segment: JV (1986) 58 142151.]
The RNA occurs in a polyhedral inner particle (composed of
proteins P1, P2, P4 and P7) which is covered with a layer
of protein P8 the whole forming the nucleocapsid (diam. ca.
60 nm). The nucleocapsid is surrounded by a phospholipid- and
protein-containing envelope (P3, P5, P6, P9, ?P10) which can be
removed (with loss of infectivity) by treatment with detergents.
An RNA polymerase (P1, P2) is associated with the capsid. The
virion also contains an enzyme (P5, ?P10) active against the host
cell wall; this enzyme seems necessary both for penetration of
the host and for the release of phage progeny.
within this sequence encodes a protein which may promote partition by binding to the plasmid at a particular site (incB ) and to
(probably) the host cell envelope [JMB (1985) 185 261272].
P1 also has a second SSR system which is responsible for the
inversion of a 4.2-kb segment (the C segment) of the P1 genome.
The C segment was first identified as a C loop analogous to
the G LOOP of bacteriophage Mu. The C segment of P1 and the
G segment of Mu are homologous (each specifies different host
ranges in different orientations), and their controlling elements
(encoded by cin in P1, gin in Mu) can complement each other
(see also RECOMBINATIONAL REGULATION). However, the inverted
repeats at each end of the C segment are not homologous
with those of the G segment. (Efficient inversion of the C
segment apparently requires an additional cis-acting sequence,
distinct from the cross-over sites cixL and cixR [PNAS (1985)
82 37763780].)
[The P1 genome: JB (2004) 186 70327068.]
bacteriophage P2 A temperate BACTERIOPHAGE (family MYOVIRIDAE) which infects Escherichia coli. The phage virion consists
of an isometric head attached to a contractile tail. Genome:
linear dsDNA (MWt ca. 22 106 ) which has 19-base STICKY
ENDS. On infection of a host cell, the DNA forms closed circular molecules which, in lysogenic infections, can integrate into
the host chromosome at a preferred site near the his operon; the
phage attachment site (attP ) occurs between genes int (encoding the P2 integrase) and ogr (see below). (cf. BACTERIOPHAGE
LAMBDA.)
P2 DNA replication occurs unidirectionally from a single
origin near the right-hand end of the genome. Replication
requires P2 genes A and B and (at least) host genes dnaB,
polC and rep; P2 gpA is a (preferentially cis-acting) DNAbinding protein. The products of DNA replication are cccDNA
monomers (i.e., concatemers are not formed). Expression of P2
late genes (which encode phage structural components) depends
on the expression of the ogr gene, which in turn depends
on P2 DNA replication. (cf. BACTERIOPHAGE P4.) During phage
assembly, the DNA monomer undergoes staggered cleavage at
a unique site (cos) to form the linear molecule with sticky ends
characteristic of the P2 virion.
bacteriophage P4 A satellite BACTERIOPHAGE (see SATELLITE
VIRUS) which infects Escherichia coli and which requires all
of the late genes of a helper phage such as BACTERIOPHAGE
P2 to complete its replication cycle. The P4 genome is linear
dsDNA (ca. 11.4 kb) with 19-nucleotide sticky ends which allow
the DNA to circularize in the host cell. P4 DNA replication
occurs bidirectionally from a single origin [JMB (1985) 182
519527]; an early P4 gene product, gpa, is required for
P4 DNA replication and is apparently a (rifamycin-resistant)
primase [JMB (1985) 182 509517]. In the absence of a helper
phage, P4 can replicate its DNA and can lysogenize its host, but
progeny virions can be formed only in the presence of a helper.
In cells co-infected with P2 and P4, P4 capsids predominate and
are assembled largely from P2 head proteins although the P4
capsid is smaller than that of P2. P4 alters the regulation of
transcription of P2 head proteins; the product of the P4 d gene
is apparently a trans-acting accessory transcription factor which
can substitute for P2 gpogr and thus circumvent the dependence
of late P2 genes on P2 DNA replication [Book ref. 118, pp.
108110].
bacteriophage P7 A BACTERIOPHAGE which is closely related to
BACTERIOPHAGE P1; however, P1 and P7 are heteroimmune and
differ in plasmid maintenance functions.
bacteriophage P22 A temperate BACTERIOPHAGE (family PODOVIRIDAE) which infects Salmonella (smooth strains). The virion
80
bacteriophage fX174
(1998) 94 147150.] In a current model, a number of pRNA
molecules form a (static) ring-shaped structure around a hole
in the phage head through which the genome is inserted; the
in length, with an axial
connector (a dodecamer of gp10, 75 A
channel) rotates, driven by ATP hydrolysis, and the threaded
(i.e. helical) DNA molecule enters the phage head like a bolt
drawn through a nut when the nut is rotated [Nature (2000) 408
745750].
Host cell lysis involves a phage-encoded peptidoglycandegrading enzyme; however, lysis also requires the product of
phage gene 14 which is apparently a LYSIS PROTEIN [JB (1993)
175 10381042].
bacteriophage f80 See STYLOVIRIDAE and LAMBDOID PHAGES.
bacteriophage f105 A temperate BACTERIOPHAGE which infects
Bacillus subtilis (see STYLOVIRIDAE). The virion consists of an
isometric head (ca. 52 nm diam.) attached to a flexible, noncontractile tail (ca. 220 nm long) which bears a baseplate with
six appendages. Genome: dsDNA (MWt ca. 26 106 ), nonpermuted, apparently with sticky ends. During lysogeny, the
phage DNA integrates at a specific attachment site in the host
chromosome but, unlike e.g. BACTERIOPHAGE l, it appears not to
circularize prior to integration, and the prophage is not circularly
permuted with respect to the virion DNA; the mechanism
of integration is not understood. On induction, f105 DNA
apparently replicates in situ, together with adjacent regions of
host DNA, and the phage DNA is subsequently excised from the
newly synthesized molecules. LFT (but not HFT) lysates have
been described; transduction appears to require that the recipient
be a f105 lysogen. [Book ref. 170, pp. 251256, 273275.]
bacteriophage fA See MICROVIRIDAE.
bacteriophage fB See MICROVIRIDAE.
bacteriophage fBA1 A temperate, tailed, dsDNA-containing
BACTERIOPHAGE isolated from Bacillus aneurinolyticus. The virions apparently have a BACTERIOCIN-like killing activity against
some strains of B. aneurinolyticus; this activity is independent
of phage gene expression (phage DNA is rapidly degraded in the
sensitive cells), and may be due to a proteinaceous component
of the intact virion [JV (1986) 59 103111]. (cf. BETACIN.)
bacteriophage fC (1) See MICROVIRIDAE. (2) See STYLOVIRIDAE.
bacteriophage fC31 A temperate bacteriophage originally isolated from Streptomyces coelicolor ; it can infect a wide range
of Streptomyces spp. Genome: dsDNA (ca. 41.5 kb) with sticky
ends. The prophage integrates in the host chromosome at a specific attachment site.
bacteriophage fCbK See STYLOVIRIDAE.
bacteriophage fD328 See STYLOVIRIDAE.
bacteriophage fEC A tailed, temperate ACTINOPHAGE whose
hosts are species of Rhodococcus; genome: linear dsDNA. fEC
is inactivated by various lipid solvents. [Book ref. 73, pp.
216218.]
bacteriophage fK See MICROVIRIDAE and BACTERIOPHAGE G4.
bacteriophage fNS11 See TECTIVIRIDAE.
bacteriophage fR See MICROVIRIDAE.
bacteriophage fW-14 A bacteriophage (family MYOVIRIDAE)
which infects and lyses certain strains of Pseudomonas acidovorans. In fW-14 DNA ca. 50% of the thymine residues are
hypermodified, occurring as a-putrescinylthymine; the hypermodified bases are apparently essential for the production of
viable progeny phages probably being required for DNA packaging [Virol. (1983) 124 152160].
bacteriophage fX174 The type species of the MICROVIRIDAE
(q.v. for morphology etc). After adsorption of fX174 to a host
cell, the ss cccDNA phage genome penetrates the cell and is
The virion adsorbs (P3, P6) to the sides of the subpolar host
pili; the f6 envelope fuses with the host outer membrane, and
the nucleocapsid minus P8 enters the host cell. Inside the cell
the phage RNA polymerase catalyses RNA synthesis; an ss
mRNA, designated l (MWt ca. 2.2 106 ), is transcribed early
and codes for P1, ?P2, P4 and P7. These four proteins form
a 120S procapsid or previrion I which incorporates progeny
dsRNA to form previrion II. (The synthesis of dsRNA is not
understood, but it occurs within a subvirion structure. A model
for the initiation of replication and transcription in bacteriophage
f6 has been proposed [Nature (2001) 410 235240].) Previrion
II synthesizes ss mRNAs m and s (MWt ca. 1.4 and 1.1 106 ,
respectively); s codes for P8 and P9, m for P3, P6 and P10 (and
possibly also P4 and P7.) Previrion II incorporates P8 to form
the complete nucleocapsid. Finally, the lipoprotein envelope
is added apparently mediated by the (non-structural) phage
protein P12; although the lipid is apparently derived from host
phospholipid, the membrane is formed in the cytoplasm and not
in contact with the cell membrane. Phage release occurs by host
cell lysis.
(Note: the name bacteriophage f6 has also been used for a
pilus-dependent dsDNA phage of Caulobacter [JV (1980) 35
949954].)
bacteriophage f29 A BACTERIOPHAGE (family PODOVIRIDAE)
which infects strains of Bacillus subtilis and those of certain
other species of Bacillus. The virion has a complex morphology: an elongated head (ca. 32 42 nm), bearing protein fibres
at each end, joined via a connector region to a short tail. Genome:
linear dsDNA (ca. 18 kb) with 6-bp terminal inverted repeats.
The 5 end of each strand in the DNA genome is formed by
a dAMP residue; each dAMP residue is linked covalently (via
a phosphodiester bond) to a serine residue in a phage-encoded
protein (gp3) a so-called terminal protein (TP). The terminal proteins are essential for initiation of replication of the f29
genome.
Replication of the linear f29 DNA is initiated at both ends
of the molecule (not simultaneously); it involves a phageencoded DNA polymerase (gp2) which has exonuclease activity
[NAR (1985) 12 12391249]. The polymerase binds to a
free molecule of the TP, and this complex localizes at the
3 end of each strand perhaps by interacting with TP at
the adjacent 5 end. The polymerase then mediates a dATPdependent reaction in which dAMP is covalently linked to the
complexed TP; this dAMP residue serves as a 3 -OH primer. The
polymerase begins strand synthesis (5 -to-3 ), and after insertion
of nucleotide 10 the polymerase and TP dissociate from one
another the TP remaining covalently bound at the 5 end of
the new strand while the polymerase continues to extend the
(DNA) primer. The polymerase is able to displace the (5 -to3 ) strand complementary to the template, and to achieve good
processivity, without help from a helicase or from other factors
[JBC (1996) 271 85098512]. Replication of the f29 genome
is an example of so-called protein priming only one example
of the strategies used for replicating a linear genome. [Protein
priming of DNA replication in phage f29: EMBO (1997) 16
25192527.] (See also ADENOVIRIDAE.)
During phage assembly, the major coat protein (gp8) is assembled with the aid of a (re-cyclable) scaffolding protein (gp7)
which is displaced as the DNA is incorporated. [Morphogenesis:
JV (1985) 53 856861.]
The packaging of DNA into the phage head requires energy
from ATP hydrolysis. It also requires certain phage-encoded
RNA molecules designated pRNA. [DNA packaging: Cell
81
bacteriophage fXahb
bacteriophage PR5 See TECTIVIRIDAE.
bacteriophage PR772 See TECTIVIRIDAE.
bacteriophage PRD1 See TECTIVIRIDAE.
bacteriophage Qb See LEVIVIRIDAE.
bacteriophage R1 See STYLOVIRIDAE.
bacteriophage R2 See STYLOVIRIDAE.
bacteriophage R17 See LEVIVIRIDAE.
bacteriophage R23 See LEVIVIRIDAE.
bacteriophage 7S See LEVIVIRIDAE.
bacteriophage S13 See MICROVIRIDAE and BACTERIOPHAGE fX174.
bacteriophage SP3 See MYOVIRIDAE.
bacteriophage SP6 A BACTERIOPHAGE which infects Salmonella
typhimurium; it has a linear dsDNA genome (ca. 43.5 kb) and
appears to resemble BACTERIOPHAGE T7 in its morphology and
development. SP6 encodes a rifamycin-resistant RNA polymerase which is synthesized shortly after infection of a host
cell. [Nucleotide sequence and expression of the cloned SP6
RNA polymerase gene: NAR (1987) 15 26532664.]
bacteriophage SP8 See MYOVIRIDAE.
bacteriophage SP50 See MYOVIRIDAE.
bacteriophage SPb See STYLOVIRIDAE and BETACIN.
bacteriophage SPO1 A virulent BACTERIOPHAGE which infects
Bacillus subtilis. The virion consists of a large isometric head,
containing >7 different polypeptides, joined via a complex
connector structure to a contractile tail which terminates in a
complex base-plate. The genome is a single molecule of linear
dsDNA, MWt ca. 108 , which contains hydroxymethyluracil.
[Review: Book ref. 170, pp. 218245.]
SPO1 is widely used in studies of transcriptional regulation
in Gram-positive bacteria. Phage genes are expressed in three
phases: early, middle and late. Early gene promoters are of
the same type as those of host genes involved in vegetative
functions, allowing transcription of early phage genes by the
(unmodified) host RNA POLYMERASE. One early gene, gene 28,
encodes a novel SIGMA FACTOR (sgp28 ) which replaces the host
s43 (formerly known as s55 ), resulting in a holoenzyme which
can recognize only phage middle promoters. Middle genes
include genes 33 and 34, the expression of which is necessary for
late gene transcription; gp33 and gp34 together replace the sgp28
in the RNA polymerase, resulting in an enzyme which in the
presence of the delta factor (see RNA POLYMERASE) recognizes
only late phage promoters, thus allowing the transcription of
late genes (which encode phage structural components). (See
also ENDOSPORE sense 1.)
bacteriophage SPO2 A temperate BACTERIOPHAGE which infects
Bacillus subtilis. Virion: an isometric head (ca. 50 nm diam.)
attached to a tail ca. 180 nm long. Genome: dsDNA, MWt ca.
26 106 . [Book ref. 170, pp. 247268 (256259).]
bacteriophage SPP1 See STYLOVIRIDAE.
bacteriophage St-1 See MICROVIRIDAE and BACTERIOPHAGE G4.
bacteriophage SV-C1 See SPIROPLASMAVIRUSES.
bacteriophage SV-C2 See SPIROPLASMAVIRUSES.
bacteriophage SV-C3 See SPIROPLASMAVIRUSES.
bacteriophage T1 See STYLOVIRIDAE.
bacteriophage T2 See T-EVEN PHAGES and MYOVIRIDAE.
bacteriophage T3 A bacteriophage (family PODOVIRIDAE) which
is very closely related to BACTERIOPHAGE T7.
bacteriophage T4 A virulent enterobacterial (linear dsDNAcontaining) BACTERIOPHAGE the best-known representative of
the T-even phages. (See entry T-EVEN PHAGES for phage structure,
nature of genome etc; see also MYOVIRIDAE.)
The T4 infection cycle is initiated when the phage attaches,
via the distal tips of its long tail fibres, to specific sites on the
bacteriophage T7
completed polynucleotide strands; HMC substitution occurs at
the level of precursor synthesis, involving hydroxymethylation
of dCTP.
Phage components are encoded by late phage genes. Heads,
tail fibres and base-plates are each assembled by separate pathways. Head assembly involves at least 20 genes. Initially, a
prohead is assembled on the host cytoplasmic membrane; the
prohead consists of a shell surrounding a central core, the latter acting as scaffolding and controlling the assembly, size and
shape of the prohead. When this structure is complete, nearly all
of its constituent proteins undergo proteolytic cleavage, resulting
in the removal of the core and the formation of a cleaved prohead. The cleaved prohead detaches from the membrane, and
the main shell protein (gp23) undergoes extensive conformational changes which result in expansion of the prohead; this step
is probably normally accompanied by DNA packaging. DNA is
packaged by the headful mechanism: one end of a linear concatemeric DNA molecule is inserted into the prohead, and the
DNA continues to be incorporated until the head is full, when the
DNA is cleaved (thus yielding the circularly permuted genome
characteristic of T4). Base-plate assembly occurs by separate
assembly of the hub and wedges (see T-EVEN PHAGES), followed
by binding of the six wedges around the hub. The tail is then
polymerized (inner tube first) on the base-plate. The completed
tail structure associates spontaneously with the DNA-containing
head, and finally the tail fibres and collar whiskers are added.
Progeny phages are released by lysis of the host cell. The
mechanism of lysis is still not fully understood, but requires
T4-coded LYSOZYME (gpe), the function of gene t (see LYSIS
PROTEIN), and possibly gp5 (the base-plate hub lysozyme see
T-EVEN PHAGES).
[Reviews on all aspects of T4: Book ref. 99.]
bacteriophage T5 See STYLOVIRIDAE.
bacteriophage T6 See T-EVEN PHAGES.
bacteriophage T7 A virulent bacteriophage of the PODOVIRIDAE
which infects Escherichia coli and other enterobacteria. Head:
isometric, ca. 60 nm diam. [capsid architecture: Virol. (1983)
124 109120]. Tail: ca. 17 nm long, with six short fibres; the
distal end of the tail adsorbs to LPS in the outer membrane
of a host cell. The T7 genome is a linear, non-permuted
dsDNA molecule (ca. 40 kb) with terminally redundant ends
(160 bp). T7 early genes constitute a single operon near the
left end of the genome; these genes are transcribed by the host
RNA polymerase and are concerned mainly with switching off
host gene transcription and switching on transcription of T7
intermediate and late genes. (The large early-gene transcript is
cleaved by host RNase III (q.v.) to give mRNAs.) Early gene
products include a protein kinase (gp0.7), which phosphorylates
and inactivates the host RNA polymerase (thus preventing
further early gene transcription), and an RNA polymerase (gp1)
which transcribes the T7 intermediate genes (concerned mainly
with T7 DNA replication) and late genes (concerned with phage
assembly and release of phage progeny by host cell lysis).
Another phage product, gp2, also binds to and inactivates host
RNA polymerase. The phage RNA polymerase is highly specific
for T7 promoters; thus, by inhibiting host RNA polymerase,
all transcriptional activity in the cell is switched to T7 DNA.
[Organization and expression of T7 DNA: CSHSQB (1983) 47
9991007.]
Replication of T7 DNA (which remains linear throughout) is
achieved mainly by proteins encoded by T7 DNA; it occurs
in three stages: (i) Initiation occurs at a single site near
the left end of the genome. (Secondary sites can be used,
host cell surface (see T-EVEN PHAGES). The tail fibres may occur
in either of two states: extended or retracted (i.e., folded back
along the tail sheath and head); infection can occur only when
the fibres are extended. Transition between the two states is
affected by conditions: retraction (and hence loss of infectivity)
is promoted by e.g. low pH, low temperature, low ionic strength,
and in some strains by the absence of the adsorption cofactor
tryptophan. Binding is initially reversible, but is followed by
irreversible binding during which the base-plate undergoes a
conformational change from a hexagonal form to an expanded,
star-shaped structure with a central opening. This in turn triggers
the contraction (by conformational change) of the tail sheath and
the penetration of the host cell envelope by the inner tail tube.
(Penetration may occur at ADHESION SITES.) The phage DNA is
then transferred through the tail inner tube to the host cell. Since
the inner tube tip appears to penetrate only as far as the outer
surface of the host cytoplasmic membrane, DNA apparently does
not enter the cytoplasm directly; uptake of the DNA by the host
cell appears to require a membrane potential and can be inhibited
by ionophores.
Infection of the host cell is followed by transcription of the
T4 DNA. This occurs in three main phases: early (immediate
early and delayed early), middle, and late; each phase occurs
at a distinct time after infection, is initiated at a distinct class
of promoters, and requires a different transcription apparatus.
The host RNA POLYMERASE is apparently used throughout, but
undergoes a series of phage-induced alterations (e.g. ADPribosylation of first one, then both, of its a subunits) which affect
its activity and affinities (e.g. for sigma factor); T4 gp55 is a
SIGMA FACTOR which is necessary for the transcription of T4 late
genes. Early effects on the host cell include the cessation of host
DNA, RNA and protein synthesis (within 25 min of infection),
unfolding of the host nucleoid, and degradation of host DNA
by phage-coded nucleases specific for cytosine-containing DNA.
The nucleotides thus released are used for the synthesis of
progeny phage DNA.
Late transcription is coupled to T4 DNA replication, which
begins ca. 5 min after infection. Replication can be initiated at
multiple origins [locations: JV (1985) 54 271277] and occurs
bidirectionally. It appears to be catalysed by a complex of phagecoded proteins (a replisome see DNA REPLICATION), including
gp43 (DNA polymerase), gp32 (an SSB protein), gp44/45/62
(DNA polymerase accessory proteins which e.g. increase polymerase processivity and affinity for DNA), gpdda (a 5 -to3 helicase), and gp41 and gp61 (involved in the priming of
Okazaki fragments). Leading strand synthesis is probably primed
initially by host RNA polymerase. Okazaki fragments in lagging strand synthesis are primed by the formation of pentaribonucleotide primers (pppApCpNpNpN, where N = any of the
4 nucleotides) by gp41 and gp61; gp41 may be analogous to
the DnaB protein of Escherichia coli (see DNAB GENE), while
gp61 may be a PRIMASE. When elongation is complete, the 3
end of the template for each lagging strand remains singlestranded; these single-stranded regions can invade homologous
regions of other phage DNA molecules, forming recombinational forks (see RECOMBINATION) and resulting in the formation
of complex, branching, concatemeric intermediates. Resolution
of the branches appears to require gp49 (T4 endonuclease VII).
Later rounds of DNA replication may be initiated at recombinational forks, allowing replication to become independent of the
(altered) host RNA polymerase. (Alteration of the RNA polymerase may prevent its recognition of origin promoters.) Modification of the DNA (glucosylation and methylation) occurs on the
83
bacteriophage Tb
is involved in the (energy-generating) light-dependent transmembrane translocation of protons. The protein part of the
bacteriorhodopsin molecule (apoprotein, bacterio-opsin) consists of seven membrane-spanning regions; the pigment RETINAL occurs within the space bounded by these seven
regions, being linked to one of them via a lysine residue.
Bacteriorhodopsin occurs in hexagonal arrays in the plane of
the membrane.
On illumination, bacteriorhodopsin undergoes a cyclical series
of changes with a periodicity of ca. 510 msec, and this
photocycling is associated with the pumping of protons from
the inner (cytoplasmic) to the outer side of the membrane, i.e.
generation of proton motive force (pmf). During photocycling
at least five photointermediates appear to be formed; these are
designated: K590 , L550 , M412 , N530 and O640 (the numbers being
wavelengths, in nm, of maximum absorption). bR568 is the lightadapted ground state.
Recent studies have clarified the mechanism, and route,
of vectorial energy-dependent transport of protons across the
membrane. Light induces the isomerization of (protonated)
retinal from all-trans to 13-cis, isomerization resulting in
deprotonation of the retinal the proton being transferred to
the asp-85 residue of the protein. Deprotonation of the retinal
causes it to change conformation, and this, in turn, modifies the
proteins conformation opening up a channel which permits
entry of a proton from the cytoplasmic side of the membrane;
this proton reprotonates residue asp-96 the proton from asp-96
having been donated to reprotonate retinal. The proton on asp85 is transferred to the exterior of the membrane; this transfer
appears to coincide with the N530 photointermediate.
When incorporated into LIPOSOMES, bacteriorhodopsin tends
(except at low pH) to adopt an orientation opposite to that in the
cytoplasmic membrane and hence to mediate inward pumping
of protons.
[Bacteriorhodopsin (overview): Nature (2000) 406 569570.
Structural changes in bacteriorhodopsin coupled to proton transport: Nature (2000) 406 645648. Structural alterations in the
M state: Nature (2000) 406 649652. Molecular mechanism of
vectorial proton translocation: Nature (2000) 406 653657.]
bacterioruberins C50 CAROTENOID pigments which occur in
members of the HALOBACTERIACEAE.
bacteriostatic (bacteristatic) Able to inhibit the growth and
reproduction of at least some types of bacteria. (cf. BACTERICIDAL.)
bacteristatic Syn. BACTERIOSTATIC.
bacterium See BACTERIA.
Bacterium
A bacterial genus which has been obsolete for
decades; various bacteria, e.g. Escherichia coli, Clostridium
chauvoei etc., were once referred to as B. coli, B. chauvoei etc.
bacterium-associated haemophagocytic syndrome (BAHS)
See HAEMOPHAGOCYTIC SYNDROME.
bacteriuria The presence of bacteria in the urine.
bacterivore Any organism (e.g. a ciliate or amoeba) which
ingests bacteria as its main or sole source of nutrients. (cf. e.g.
DETRITIVORE.)
bacterization The process of coating seeds, tubers etc. with
certain bacteria (e.g. Azotobacter), prior to planting, with the
object of improving plant growth.
bacteroid A bacterium-like cell or a modified bacterial cell see
e.g. ROOT NODULES. (In an ACTINORRHIZA, bacteroid may refer
e.g. to a senescent hyphal fragment.)
Bacteroidaceae A family of (typically) Gram-negative, anaerobic, chemoorganotrophic, asporogenous, motile and non-motile,
Baculoviridae
typically rod-shaped or filamentous bacteria, some of which
are pathogenic in man and other animals. Genera: ACETIVIBRIO,
ANAEROBIOSPIRILLUM, ANAEROVIBRIO, BACTEROIDES, BUTYRIVIBRIO, FUSOBACTERIUM, LACHNOSPIRA, LEPTOTRICHIA, PECTINATUS,
SELENOMONAS, SUCCINIMONAS, SUCCINIVIBRIO and WOLINELLA. In
some of these organisms (e.g. Acetivibrio, Butyrivibrio, Lachnospira) the CELL WALL appears to resemble the Gram-positive
(rather than Gram-negative) type of wall; since these organisms
give a negative or variable reaction in the Gram stain (at least
under some conditions) they have been grouped with the frankly
Gram-negative genera [Book ref. 22, pp. 602662].
Bacteroides
A genus of Gram-negative bacteria (family
BACTEROIDACEAE) which occur e.g. in the RUMEN and in the
mouth and intestinal tract in man and other animals; some
species are opportunist pathogens, being isolated from abscesses
and other types of lesion (see e.g. FOOT-ROT; PNEUMONIA
(f); SCALD). (See also ANAEROBIC DIGESTION; TERMITEMICROBE
ASSOCIATIONS; WETWOOD.) Cells: typically rods or filaments, nonmotile or peritrichously flagellated, sometimes with central or
terminal swellings or vacuoles. Some species form a dark or
black pigment. [Black-pigmented strains from animals: JAB
(1983) 55 247252.] Metabolism is typically fermentative,
though some strains can carry out FUMARATE RESPIRATION in
media containing haemin electron donors including formate
and H2 . Most species (fermentative, saccharoclastic or
saccharolytic species) typically attack a range of sugars,
producing a mixture of products which may include acetic,
formic, lactic, propionic and succinic acids; such species usually
use or need CO2 which is assimilated by the reductive
carboxylation of succinate to 2-oxoglutarate. Other species
attack sugars weakly, or not at all, but utilize peptones
with the formation of mixtures of either small amounts of
e.g. acetic, formic, lactic and succinic acids, or mixtures of
larger amounts of e.g. acetic, butyric, propionic and succinic
acids isobutyric and isovaleric acids being formed whenever
butyric acid is formed. Primary isolation may be carried out
on media containing e.g. peptone, yeast extract, haemin and
menaquinone under at least 5% CO2 . GC%: ca. 2861. Type
species: B. fragilis.
B. endodontalis. A non-saccharolytic, black-pigmented species isolated from the dental root canal [IJSB (1984) 34
118120].
B. fragilis (formerly Fusiformis fragilis). Cells (in glucose
broth): non-motile round-ended rods, 0.81.3 1.68.0 m.
Catalase +ve (most other species are catalase ve). Saccharolytic; in haemin-containing media some strains form a b-type
cytochrome and can carry out fumarate respiration. On horse- or
rabbit-blood agar colonies are typically smooth, round, entire,
low convex, grey and non-haemolytic; some strains produce
clear (b) haemolysis. Optimum growth temperature: 37 C.
B. fragilis may be sensitive to e.g. CEFOXITIN and clindamycin
(see LINCOSAMIDES). (The B. fragilis group commonly includes
former subspecies of B. fragilis which are currently classified as species: B. distasonis, B. ovatus, B. thetaiotaomicron and
B. vulgatus.)
B. melaninogenicus. A saccharolytic species which forms a
black pigment (a haem derivative) and which has SOD activity;
it occurs e.g. in the human mouth.
B. nodosus. A non-motile, non-saccharolytic species which
causes foot-rot in sheep. [Surface structure and virulence of
B. nodosus: JGM (1983) 129 225234.]
B. ochraceus. See CAPNOCYTOPHAGA.
B. pneumosintes (formerly Dialister pneumosintes). A nonsaccharolytic species which occurs e.g. in the human nasopharynx and which may be a secondary invader in upper respiratory
tract infections. Cells: typically 0.20.4 0.30.6 m.
B. ruminicola. A saccharolytic species which ferments a wide
range of carbohydrates, including e.g. cellobiose and starch; it
occurs in the RUMEN.
B. succinogenes. A saccharolytic rumen species which attacks
relatively few sugars but which can utilize cellobiose and
cellulose; unlike B. ruminicola, this species does not digest
gelatin or hydrolyse aesculin.
B. termitidis (formerly Sphaerophorus siccus var. termitidis).
A saccharolytic species which occurs in the intestinal tract in
termites.
Other species: B. amylophilus, B. asaccharolyticus, B. bivius,
B. buccae, B. capillosus, B. coagulans, B. corporis, B. denticola,
B. disiens, B. distasonis, B. eggerthii, B. furcosus, B. gingivalis,
B. gracilis, B. hypermegas, B. intermedius, B. levii, B. loescheii,
B. macacae, B. microfusus, B. multiacidus, B. oralis, B. oris,
B. ovatus, B. praeacutus (cf. TISSIERELLA), B. putredinis, B. splanchnicus, B. thetaiotaomicron, B. uniformis, B. ureolyticus,
B. vulgatus and B. zoogleoformans.
[Book ref. 22, pp. 604631; Bacteroides of the human lower
intestinal tract: ARM (1984) 38 293314.]
Bacto The designation of products of Difco Laboratories Inc.,
Detroit, USA.
bactoprenol (undecaprenol) In bacteria: a lipid-soluble, membrane-bound polyprenol consisting of a linear chain of 11
unsaturated isoprene units:
H[CH2 .C(CH3 )=CH.CH2 ]11 OH
Bactoprenol phosphate acts as a carrier in the synthesis of a
number of cell envelope and extracellular polymers: e.g., PEPTIDOGLYCAN, LIPOPOLYSACCHARIDE, TEICHOIC ACIDS and certain CAPSULE polymers; it apparently facilitates the transfer of lipophobic
sugar residues across the cytoplasmic membrane. (cf. DOLICHOL;
see also TUNICAMYCIN.)
Baculoviridae A family of ccc dsDNA-containing VIRUSes which
infect arthropods (particularly insects of the Diptera, Hymenoptera and Lepidoptera). Baculovirus virions are structurally
complex, consisting of one or more nucleocapsids within an
envelope; virions containing one nucleocapsid per envelope are
rod-shaped, ca. 200400 4060 nm. The genome is nonsegmented circular supercoiled dsDNA, MWt ca. 58110 106 .
The family is divided (on morphological criteria) into three
subgroups: A (the NUCLEAR POLYHEDROSIS VIRUSES, NPVs), B
(the GRANULOSIS VIRUSES, GVs), and C. (cf. POLYDNAVIRIDAE.)
The NPVs and GVs are characterized by the formation of intracellular crystalline protein occlusion bodies within which virions
are embedded; the NPVs form polyhedral intranuclear occlusion
bodies (called POLYHEDRA), each containing many virions, while
the GVs form ellipsoidal or round-ended rod-shaped occlusion
bodies (called granules or capsules), each containing only one
(rarely two) virions. The matrix proteins of both types of occlusion body (called polyhedrin, or polyhedrin in NPVs and granulin in GVs) are closely related in structure and function [review:
JGV (1986) 67 14991513], but are apparently unrelated to the
polyhedrins of the CYTOPLASMIC POLYHEDROSIS VIRUS GROUP. In
contrast to the NPVs and GVs, baculoviruses of subgroup C do
not form occlusion bodies; viruses of this subgroup have been
observed in various arthropods (insects, arachnids, crustacea),
the type species of the subgroup being Oryctes rhinoceros virus
(from the coconut palm rhinoceros beetle).
85
baculoviruses
An insect becomes infected with an NPV or GV when
it ingests an occlusion body; the polyhedrin dissolves in the
alkaline contents of the insects midgut, releasing virions which
then infect cells of the midgut. Non-occluded virions produced
in these cells bud through the plasma membrane of the midgut
cells and are disseminated via the haemolymph, subsequently
infecting cells of a wide range of tissues. The virion-containing
occlusion bodies are formed late in infection, and are eventually
released by the death and dissolution of the insect host.
Baculoviruses have been extensively used for the BIOLOGICAL
CONTROL of insect pests; they are particularly suitable for
this purpose since they have no apparent relationship with
any other known animal or plant viruses (and are therefore
deemed unlikely to infect mammals or plants), and they can
be lethal for and spread rapidly among insects in nature.
Thus, e.g., NPVs have been used to control the European
pine sawfly (Neodiprion sertifer ) and European spruce sawfly
(Gilpinia hercyniae), GVs have been used against the Small
White butterfly (Artogeia (= Pieris) rapae, a pest of crucifers),
and Oryctes rhinoceros virus has been used successfully to
control the coconut palm rhinoceros beetle.
Since NPVs and GVs produce large quantities of polyhedrin/granulin in infected cells, the genomes of these viruses are
of interest as vectors for the introduction and high-level expression of foreign genes in insects or insect cell cultures; e.g., a
recombinant baculovirus containing a human a-interferon gene
linked to the polyhedrin promoter yielded large quantities of
a-interferon in silkworms [Nature (1985) 315 592594].
baculoviruses Viruses of the BACULOVIRIDAE.
Badhamia See MYXOMYCETES.
BaeI See RESTRICTION ENDONUCLEASE (table).
baeocyte A small, spherical reproductive cell (diam. ca. 23 m)
formed by members of section II of the CYANOBACTERIA.
Baeocytes (formerly termed endospores) are produced by
multiple fission of a vegetative cell which is enclosed in a fibrous
layer external to the outer membrane of the cell wall; numerous
baeocytes are released on rupture of the fibrous layer. A baeocyte
enlarges, without division, until it reaches the size of a vegetative
cell, this growth being accompanied by a progressive thickening
of the fibrous outer layer. Gliding motility may be exhibited
initially by those baeocytes which lack a fibrous outer layer at
the time of their release.
Baeomyces A genus of LICHENS (order LECANORALES); photobiont: e.g. Myrmecia. Thallus: crustose to squamulose, often
sorediate. Fruiting bodies are non-lichenized, stalked, convex
hymenial discs resembling miniature mushrooms (cf. PODETIUM).
Species occur on soil, rocks etc.
BAF See SEWAGE TREATMENT.
bagassosis An EXTRINSIC ALLERGIC ALVEOLITIS associated with
inhalation of the dust of sugar cane waste (bagasse); certain bacteria (e.g. Thermoactinomyces sacchari ) have been implicated.
BAHS (bacterium-associated haemophagocytic syndrome) See
HAEMOPHAGOCYTIC SYNDROME.
bakanae disease (foolish seedling disease; foolish rice) A
disease of rice caused by Gibberella fujikuroi (Fusarium
moniliforme) and characterized by conspicuous elongation of
the plant stems (internodes) followed by wilting. The symptoms
are believed to be due to the effects of GIBBERELLINS produced
by the pathogen. (See also CEREAL DISEASES.)
bakers yeast A specialized strain of Saccharomyces cerevisiae
which is capable of rapid fermentative activity in dough (see
BREAD-MAKING), i.e., under conditions of low oxygen tension,
low water activity, and high osmotic pressure. The yeast is manufactured by batch culture (in a medium containing molasses,
Bartonella
barophiles) die at a temperature-dependent rate. Barophilic
bacteria in seas and oceans occur both in the nutrient-poor
seawater and in the relatively nutrient-rich guts of invertebrates
(e.g. holothurians sea cucumbers); those occurring in cold
regions (<4 C) are heterotrophic bacteria (cf. HYDROTHERMAL
VENT). [Reviews: ARM (1984) 38 487514; MS (1986) 3
205211.] (See also BAROTOLERANT.)
barophilic Having the characteristics of a BAROPHILE.
barosensitive See BAROTOLERANT.
barotolerant (baroduric) Refers to an organism which can grow
at elevated pressures (up to ca. 400600 atmospheres; 1 atm =
101.325 kPa) but which grows optimally at atmospheric pressure
(cf. BAROPHILE); many bacteria (including e.g. Escherichia coli
and Pseudomonas aeruginosa) are barotolerant, but some (e.g.
Vibrio parahaemolyticus) cannot survive for long even under
relatively low pressures (e.g. ca. 200 atm) and are termed
barosensitive.
The inhibitory effect on barotolerant organisms of pressures
greater than ca. 400600 atm appears to be due, at least partly, to
inhibition of certain aspects of PROTEIN SYNTHESIS specifically,
the binding of amino acyl-tRNAs and translocation. In a number
of organisms the susceptibility of protein synthesis to pressure
has been linked with the 30S ribosomal subunit; interestingly,
increased barotolerance occurs in those strains of E. coli which
have become resistant to streptomycin owing to a mutation
affecting the 30S subunit.
barren kinetosome See CILIFEROUS.
barrier filter See MICROSCOPY (e).
Barritts method See VOGESPROSKAUER TEST.
Barrouxia See EIMERIORINA.
Bartonella A genus of Gram-negative, oxidase-negative bacteria
(family BARTONELLACEAE) within the alpha subgroup of Proteobacteria; the cells are small, typically capnophilic, fastidious
rods which can usually be grown aerobically on blood-agar in
the presence of 5% carbon dioxide [guidelines for the practical
identification of isolates: JCM (1993) 31 23812386].
The genus now includes several species which have been
imported from the (former) genus Rochalimaea [IJSB (1993)
43 777786].
B. bacilliformis (the type species) is the causal agent of
BARTONELLOSIS in man (the only natural host); the bacterium
is a small bacillus or pleomorphic coccobacillus, commonly ca.
13 m in length, which, in culture, bears one or more flagella
at one pole and divides by binary fission; it is transmitted by
sandflies, and occurs in or on erythrocytes, and in endothelial
cells, in infected persons.
B. clarridgeiae has been associated with cat scratch disease
[JCM (1997) 35 18131818].
B. elizabethae (formerly Rochalimaea elizabethae) has been
isolated from a case of endocarditis [JCM (1993) 31 872881].
B. henselae (formerly Rochalimaea henselae) has been associated with various types of disease, including e.g. cutaneous
bacillary angiomatosis; this disease (which occurs mainly in
the immunocompromised) involves reddish-coloured, typically
nodular lesions which may ulcerate. (R. quintana can also give
rise to the disease.)
B. quintana (formerly Rochalimaea quintana) is the causal
agent of TRENCH FEVER; the cells are small rods, and the organism
is aerobic and capnophilic.
B. vinsonii (formerly Rochalimaea vinsonii ) is parasitic in
voles (the Canadian vole agent); it is not capnophilic.
[Diseases caused by Bartonella spp: RMM (1995) 6
155164.]
BASIDIOSPORE.)
Bartonellaceae
to each other. (Other combinations (AA, GT, AC, GG,
AG) can occur under certain circumstances [Nature (1976)
263 285289] but these are less stable than the classical pairs.)
Classical base-pairing is responsible for holding together the
strands in dsDNA (see DNA) or in dsRNA (e.g. in certain
viruses); it is also involved e.g. in ordering the sequence of
nucleotides in DNA REPLICATION and TRANSCRIPTION.
base ratio (dissymmetry ratio) Of microbial DNA: the ratio
(A + T)/(G + C) in which A, T, G and C represent relative molar
amounts of adenine, thymine, guanine and cytosine, respectively.
(cf. GC%.) Species with a base ratio >1 may be called AT types;
GC types have a base ratio <1.
basic dye See DYE.
basic fuchsin See FUCHSIN.
basic orange Syn. ACRIDINE ORANGE.
basic replicon (1) The smallest part of a replicon which encodes
all the functions necessary for replication.
(2) As (1), above, with the added constraint that replication
maintains the wild-type COPY NUMBER [Book ref. 161, p. 202].
Basidiobolus See ENTOMOPHTHORALES.
basidiocarp A fruiting body of a basidiomycete.
basidiole (1) An immature BASIDIUM prior to the appearance of
the sterigmata. (2) An aborted basidium. (3) A sterile cell which
is similar in appearance to an immature basidium.
basidiolichen A lichen (see LICHENS) in which the mycobiont is
a basidiomycete.
basidiomycetes Fungi of the BASIDIOMYCOTINA.
Basidiomycotina (the basidiomycetes) A subdivision of fungi
(division EUMYCOTA) characterized by the formation of sexually derived spores (BASIDIOSPORES) on basidia (see BASIDIUM).
The basidiomycetes are typically terrestrial saprotrophs or parasites; they include e.g. mushrooms, puffballs, stinkhorns, and
the (parasitic) rust and smut fungi. A few basidiomycetes are
marine organisms (see e.g. NIA). In most species the thallus
is a well-developed septate mycelium which often has CLAMP
CONNECTIONS (see also DOLIPORE SEPTUM); some basidiomycetes
can occur in a yeast-like (unicellular) phase (see FILOBASIDIACEAE) as can certain fungi which appear to be the anamorphs
of basidiomycetes (see e.g. SPOROBOLOMYCETACEAE).
In the typical life cycle, the germination of a basidiospore
leads to the development of a septate mycelium consisting of
uninucleate, haploid cells. At some stage the thallus enters
DIKARYOPHASE (see also HYPHA), and eventually karyogamy and
MEIOSIS occur in the developing basidium which typically
gives rise to four (haploid) basidiospores.
Classes: GASTEROMYCETES, HYMENOMYCETES, UREDINIOMYCETES, USTILAGINOMYCETES.
Basidiophora
A genus of fungi (order PERONOSPORALES) in
which the sporangiophores resemble basidia, and the sporangia
are borne on short sterigmata; the organisms include parasites
of the ornamental aster and of members of the Compositae.
basidiospores Sexually-derived, typically uninucleate and haploid SPORES formed on basidia (see BASIDIUM) by fungi of
the BASIDIOMYCOTINA. According to species, basidiospores may
be any of various shapes and sizes, and either pigmented or
non-pigmented. In many basidiomycetes the basidiospores are
BALLISTOSPORES, while in some (e.g. smut fungi) they are
STATISMOSPORES. (cf. GASTEROID BASIDIOSPORE.) On germination,
a basidiospore commonly gives rise to a germ tube, but in some
cases GERMINATION BY REPETITION may occur.
Dispersal of basidiospores. In agarics with aequihymeniiferous lamellae (see LAMELLA), the ballistospores are projected
more or less horizontally for ca. 0.10.2 mm before gravity
batch culture
four basidiospores per basidium; in many smut fungi the
basidium may give rise to an indefinite number of basidiospores
following mitotic divisions within the metabasidium.
[Review: BBMS (1983) 17 8294.]
basionym (basonym) The name of the species whose specific
epithet is included in a new combination (see COMB. NOV.).
basipetal development Development from the tip towards the
base or point of attachment; e.g., in a chain of basipetally
developing spores the first-formed spores occupy positions
in the terminal or distal parts of the chain, while spores
formed later occupy the more proximal positions. (cf. ACROPETAL
DEVELOPMENT.)
basonym Syn. BASIONYM.
basophil A PMN (q.v.) which can respond to certain stimuli
e.g. by rapidly secreting vasoactive products; it is primarily
a circulatory cell, and is important e.g. in immediate-type
hypersensitivity reactions. As in the MAST CELL, with which
it shares many characteristics, the basophil surface contains
e.g. many high-affinity receptor sites for the Fc portion of
IgE antibodies, and its (basophilic) cytoplasmic granules also
contain substances such as HISTAMINE and SEROTONIN; stimuli
which cause activation and degranulation lead to the secretion
of various products and to the formation of e.g. SUPEROXIDE and
H2 O2 . (See also JONESMOTE SENSITIVITY.)
batch culture (closed culture) A form of CULTURE (sense 2)
in which a given volume of liquid medium is inoculated with
cells (e.g. bacteria) capable of growth in that medium, and
the inoculated medium is incubated for an appropriate period
of time; cells growing under these conditions are exposed to
a continually changing environment due e.g. to the gradual
consumption of nutrients and the accumulation of metabolic
wastes (cf. CONTINUOUS CULTURE and FED BATCH CULTURE).
The growth curve (see GROWTH) obtained by monitoring a
batch culture commonly exhibits a sequence of four main phases
of growth. In the lag phase the growth rate i.e., the rate of
increase in cell numbers (or biomass) is initially minimal but
subsequently rises to a value dictated e.g. by the prevailing
conditions (e.g. temperature, concentration of nutrients etc). The
length of the lag phase is influenced by the cultural history of
the cells in the inoculum. For example, if slowly dividing cells
from a nutrient-poor environment are transferred to a nutrientrich medium which can support a higher rate of growth, there is
usually a relatively long lag phase during which time the cells
become adapted to the new environment; during this period of
adaptation the cells exhibit unbalanced GROWTH. Subsequently,
growth occurs at a new, higher rate permitted by the higher
levels of nutrients. A long lag phase may also occur e.g. if the
carbon source in the new medium differs from that previously
used by the cells. (cf. DIAUXIE.) When actively dividing cells are
transferred to a medium which offers conditions similar to those
under which the cells were previously growing, a lag phase is
not observed.
At the end of the lag phase the cells enter the exponential
(= logarithmic or log) phase of growth in which, for a given
organism, the growth rate is both constant and maximal for the
particular growth conditions. In this phase there is an exponential
increase in cell numbers (and biomass); this type of growth is
referred to as balanced GROWTH. (See also TROPHOPHASE.)
In the stationary phase the growth rate declines and eventually
reaches zero. (See also IDIOPHASE.)
In the death phase the number of viable cells in the culture
(maximal in the stationary phase) declines.
initiates a vertical fall; the spores on a given basidium are commonly discharged in rapid succession (within seconds or minutes
of one another). In these agarics the shape of the lamella facilitates spore dispersal spores from the more proximal parts of
the lamella being able to fall vertically even when the lamellae
are orientated several degrees from the vertical.
In e.g. Coprinus spp the inaequihymeniiferous lamellae occur
close together on the pileus, and the shape of the lamellae
does not facilitate dispersal of the ballistospores. However, in
some species cystidia (see CYSTIDIUM) may serve to hold apart
adjacent hymenial surfaces. In other species the process of
autodigestion is an aid to spore dispersal; autodigestion involves
the progressive liquefaction of the lamellae, beginning at the free
edge of the lamella and progressing towards the pileus as fresh
crops of basidia become mature. Thus, spores discharged by
a given basidium need fall for only a short distance between
adjacent lamellae before becoming free of the fruiting body.
See also e.g. CYATHUS, LYCOPERDALES, SPHAEROBOLUS.
basidium (pl. basidia) A microscopic, unicellular or multicellular structure which gives rise to the sexually-derived spores
(BASIDIOSPORES) in fungi of the BASIDIOMYCOTINA; basidiospores
are formed externally, i.e., as extrusions, on the basidium (but
see TETRAGONIOMYCES). In some basidiomycetes (e.g. HYMENOMYCETES) the basidia are formed in a layer on specialized fertile
tissue (see HYMENIUM), while in others (e.g. UREDINIOMYCETES)
they are formed individually from germinating spores.
In many species the basidium is a simple, cylindrical or
clavate structure which gives rise to (usually) four apically and
symmetrically situated basidiospores, each basidiospore commonly being borne on a small, narrow protrusion (STERIGMA). In
other species the basidium may be apically bifurcate, each fork
(sterigma) bearing a single terminal basidiospore (as in members of the DACRYMYCETALES), or it may be divided, apically,
into four substantial finger-like protrusions (sterigmata), each
bearing a terminal basidiospore (as in members of the TREMELLALES). A basidium which is not divided, internally, by septa is
called a holobasidium; such basidia are formed by members of
the HOLOBASIDIOMYCETIDAE. A basidium which is divided, internally, by transverse or longitudinal septa (as e.g. in Auricularia
and Tremella, respectively) is called a phragmobasidium; such
basidia are formed by members of the PHRAGMOBASIDIOMYCETIDAE and of the UREDINIOMYCETES and USTILAGINOMYCETES.
Basidium formation. A simple holobasidium typically develops from a terminal dikaryotic hyphal cell within a hymenium;
the boundary between this cell and the parent hypha is often
marked by a CLAMP CONNECTION. Within the developing basidium, karyogamy and MEIOSIS commonly give rise to four haploid
nuclei. (See also METABASIDIUM and PROBASIDIUM.) Four small
protuberances (sterigmata) then form at the apical (free) end of
the developing basidium, and the terminal part of each sterigma
swells to form a basidiospore initial; one nucleus migrates into
each initial, and the basidiospores are subsequently delimited.
In some species mitotic division occurs within the developing
basidiospores; in such cases either binucleate basidiospores are
formed, or uninucleate basidiospores are formed after one daughter nucleus from each pair has returned to the basidium.
In rust and smut fungi, the basidium typically develops from
a short germ tube which arises from the teliospore. In some
cases a diploid nucleus passes from the teliospore into the germ
tube and undergoes meiosis; the structure which develops (the
metabasidium, or promycelium) is septate in many species and
(in rusts, and in many smut fungi) it gives rise to basidiospores
both apically and laterally. Rust fungi characteristically form
89
batch retort
batch retort In CANNING: a vessel within which filled, sealed
cans (or other containers) undergo heat treatment in a batchtype process (cf. COOKERCOOLER). The cans are subjected to
saturated steam under pressure or to an airsteam mixture, or (in
an overpressure retort) are submerged in heated water under an
air pressure of up to ca. 250 kPa. In some batch retorts (e.g. the
Konservomat) the load is agitated to facilitate heat penetration.
bating (of hides) See PROTEASES.
Batrachospermum See RHODOPHYTA.
Battarrea See GASTEROMYCETES (Tulostomatales).
Battey bacillus Strain(s) of Mycobacterium intracellulare or,
loosely, strain(s) of related species (including M. avium).
Bayers junction (Bayers patch) See ADHESION SITE.
Bayleton See TRIADIMEFON.
BB-transhydrogenase See TRANSHYDROGENASE.
BCDF (immunol.) See LYMPHOKINES.
BCF Bioconcentration factor: a measure of the degree to which
a compound (commonly a xenobiotic), present in an aquatic
environment, is accumulated in the biomass of organisms (e.g.
algae) living in that environment. BCF = Co /Cw where Co =
concentration of the compound in the organisms, and Cw is the
concentration of the compound in the water. (See e.g. TBTO.)
BCG Bacille (bacillus) CalmetteGuerin: an attenuated strain of
Mycobacterium bovis used e.g. as a vaccine against TUBERCULOSIS. The vaccine often gives protection against e.g. tubercular
meningitis in childhood but in a number of studies it has
failed to protect against pulmonary tuberculosis [Lancet (1990)
335 10161020]; moreover, it may produce disseminated infections in the immunocompromised (e.g. AIDS patients). In some
instances, BCG has provided some protection against LEPROSY.
[Mycolic acids in BCG substrains: JGM (1984) 130
27332736.]
(See also ESAT-6.)
BCGF (immunol.) See LYMPHOKINES.
Bchl Bacteriochlorophyll: see CHLOROPHYLLS.
BclI A RESTRICTION ENDONUCLEASE from Bacillus caldolyticus;
T/GATCA.
BCNU See N-NITROSO COMPOUNDS.
Bd (buoyant density) See CENTRIFUGATION and GC%.
BD-type starter See LACTIC ACID STARTERS.
bdellocyst See BDELLOVIBRIO.
bdelloplast See BDELLOVIBRIO.
Bdellospora See ZOOPAGALES.
Bdellovibrio A genus of aerobic Gram-negative bacteria which
are characteristically predatory on other bacteria (cf. VAMPIROVIBRIO); they occur worldwide in soil and sewage, and in freshwater
and marine habitats. On primary isolation all strains are obligately parasitic on certain Gram-negative bacteria, including e.g.
Aquaspirillum serpens, Escherichia coli, Pseudomonas spp, and
Rhodospirillum rubrum the range of prey species varying with
the strain of Bdellovibrio; prey-independent, cultivable strains
can develop from strictly predatory strains, and some strains are
facultatively predatory. The predatory strains exhibit a biphasic life cycle: the predatory phase (in which the non-growing
cells search for prey) alternating with a phase of growth and
reproduction in the periplasmic space of a host cell. Predatory
cells of Bdellovibrio are vibrioid, 0.20.5 0.51.4 m, each
having a single polar sheathed flagellum (the sheath being continuous with the outer membrane); cells of prey-independent
strains may be larger and non-motile, and may form a yellowish pigment. All strains are chemoorganotrophs. Growth occurs
optimally at 2830 C, and metabolism is respiratory (oxidative). Three species are recognized [Book ref. 22, pp. 118124]:
benign foot-rot
beet cryptic viruses See CRYPTIC VIRUSES.
beet curly top virus See GEMINIVIRUSES.
beet leaf curl virus See RHABDOVIRIDAE.
beet mild yellowing virus See LUTEOVIRUSES.
beet mosaic virus See POTYVIRUSES.
beet necrotic yellow vein virus (BNYVV) A virus which can
cause severe disease (rhizomania) in sugar beet (Beta vulgaris);
it is transmitted by the fungus Polymyxa betae which is also
responsible for the persistence of the virus in the soil. BNYVV
may belong to the furovirus group see SOIL-BORNE WHEAT
MOSAIC VIRUS. (cf. TOBAMOVIRUSES.) [BNYVV RNA: JGV (1985)
66 345350.]
beet western yellows virus See LUTEOVIRUSES.
beet yellow net virus See LUTEOVIRUSES.
beet yellow stunt virus See CLOSTEROVIRUSES.
beet yellows virus group Syn. CLOSTEROVIRUSES.
Beggiatoa A genus of GLIDING BACTERIA (see CYTOPHAGALES);
species are widespread e.g. in freshwater, estuarine and marine
waters and sediments, in the rice rhizosphere, and in activated
sludge. The organisms are non-sheathed, non-pigmented, multicellular filaments (trichomes) which form necridia and hormogonia; according to species, the trichomes are 1 to >50 m
in diameter. The organisms appear to be chemoorganotrophic
heterotrophs, although at least some strains may be able to grow
mixotrophically using sulphide as an electron donor; refractile
intracellular granules of sulphur (located between cytoplasmic
membrane and cell wall) are formed in the presence of sulphide.
Metabolism is respiratory, and a complete TCA cycle is present.
Most strains can use acetate and/or lactate as the sole source
of carbon; none can use hexoses. The main storage product is
poly-b-hydroxybutyrate; volutin is also formed. [Review: ARM
(1983) 37 341354.]
Beggiatoaceae See CYTOPHAGALES.
Beijerinckia A genus (incertae sedis) of Gram-negative, aerobic,
catalase-positive, chemoorganotrophic, asporogenous bacteria
which occur e.g. in the phyllosphere and in soils (particularly
in the tropics). Cells: typically round-ended rods, ca. 0.51.5
1.74.5 m, peritrichously flagellated or non-motile; division
involves constriction. Each cell characteristically contains two
PHB-containing polar bodies. In some species each cell may be
encysted, or several cells may occur within a single capsule.
Metabolism is respiratory (oxidative), with O2 as terminal
electron acceptor. NITROGEN FIXATION is carried out under both
atmospheric and microaerobic conditions; in many strains N2
is used in preference to NO3 . All strains can utilize glucose,
fructose and sucrose as carbon sources; peptone does not
support growth. Slime (sometimes elastic) is commonly formed,
particularly on agar under N2 -fixing conditions. Colonies are
often some shade of pink, or orange to pale brown. No pellicle
is formed on liquid media. Optimum growth temperature:
2030 C; no growth at 37 C. Growth can occur within the pH
range ca. 310. GC%: ca. 5561. Type species: B. indica; other
species: B. derxii, B. fluminensis and B. mobilis. [Book ref. 22,
pp. 311321.]
bell morels The fruiting bodies of VERPA spp.
belladonna mottle virus See TYMOVIRUSES.
benalaxyl See PHENYLAMIDE ANTIFUNGAL AGENTS.
Beneckea An obsolete bacterial genus, members of which are
now included in the genus VIBRIO.
benign (med.) (1) (of disease) Mild; self-limiting; not recurrent.
(2) (of tumours) Not MALIGNANT (sense 2).
benign enzootic paresis Syn. TALFAN DISEASE.
benign foot-rot (of sheep) See SCALD.
BIAcore
of other herpesviruses). In culture they typically give rise to
enlarged, rounded cells (cytomegalic cells) and slowly spreading
foci of cell lysis. DNA-containing inclusion bodies may be seen
in the nuclei and sometimes in the cytoplasm of infected cells.
Typically, the host range for a given virus is narrow and is often
restricted to a single species. Latent infection can be established
in cell cultures and in vivo.
HCMV (often truncated to CMV) is a large herpesvirus
with a linear dsDNA genome of MWt ca. 1.5 108 containing
terminal and internal repeated sequences; the genome encodes
a number of structural and regulatory proteins. Each virion
consists of the DNAprotein core, a capsid, and an external
lipoprotein envelope bearing surface projections, the region
between envelope and capsid (the tegument) containing several
virus-encoded proteins.
In the replication cycle of HCMV, the virion initially fuses
with the cell membrane of the target cell, and the (unenveloped)
virus migrates towards the nucleus. Viral DNA is replicated in
the nucleus, and virus-encoded proteins are synthesized in the
cytoplasm; the nucleocapsid is assembled in the nucleus.
HCMV genes are transcribed in strict temporal sequence.
The immediateearly genes (expressed within 24 hours
of infection) encode regulatory proteins that are needed for
synthesis of early and late genes. The early gene products
include a DNA polymerase. Late gene products include capsid
proteins.
Culture of human CMV is carried out in human fibroblasts.
(See also SHELL VIAL ASSAY.) In vivo, replication appears to occur
primarily in epithelial cells (e.g. in salivary glands, kidneys);
HCMV is also known to infect peripheral blood leukocytes and
haematopoietic progenitor cells.
Infection with HCMV is endemic in human populations
world-wide, but in most cases it is asymptomatic; primary infection may be followed by viral persistence which may take
the form of low-level replication or latent infection. (The site
of latency is currently unknown.) However, the virus is e.g.
a common cause of congenital viral infections, and sometimes causes a disease resembling INFECTIOUS MONONUCLEOSIS. HCMV-mediated disease appears to occur most commonly
among the immunocompromised (e.g. immunosuppressed transplant patients and AIDS patients) and in those with an immature
immune system (e.g. neonates). Typically, HCMV-mediated disease is associated with conditions such as fever, hepatitis and
leukopenia. (See also CYTOMEGALIC INCLUSION DISEASE.)
[Epidemiology and transmission of HCMV: JID (1985)
152 243248. Molecular biology and immunology of HCMV
(review): Bioch. J. (1987) 241 313324. Occupational risk of
HCMV: RMM (1994) 5 3338. HCMV in haematological disease: BCH (1995) 8 149163.]
The laboratory diagnosis of HCMV can be achieved in <24
hours e.g. by SHELL VIAL ASSAY or by serological or nucleic acidbased techniques [diagnosis of HCMV by detection of antigen
and DNA: RMM (1994) 5 265276]. A NASBA-based procedure
has been used for detecting the transcript of a late HCMV gene
in order to monitor transplant patients at risk from HCMVrelated disease [JCM (1998) 36 13411346].
In recent years, two more herpesviruses have been added
to the Betaherpesvirinae: human (beta) herpesvirus 6 (human
herpesvirus 6, HHV6) and human (beta) herpesvirus 7 (human
herpesvirus 7, HHV7).
HHV6 has been identified as a causal agent of EXANTHEM
SUBITUM, and is able to cause severe morbidity in immunocompromised patients; it is also a possible causal agent of e.g.
lymphoma and leukaemia.
biofilm
time, and a standard curve is constructed by plotting the amount of
growth against the concentration of pantothenic acid; the standard
curve can then be used to quantify an unknown concentration of
pantothenic acid. Clearly, a medium must not contain substance(s)
which allow the test organism to bypass the restriction on growth
imposed by the limiting concentration of the assayed substance;
in the case of BIOTIN bioassay, for example, the presence of
pimelic acid in the medium may circumvent the requirement for
biotin and permit growth of the test organism. (See also FOLIC
ACID; METHANOBREVIBACTER; NICOTINIC ACID; VITAMIN B12 ; cf.
BIOAUTOGRAPHY.)
Bioassay is also used e.g. for measuring concentrations of
antimicrobial agents, and for assaying the pathogenicity of
entomopathogenic microorganisms by determining their effect
on susceptible insect populations.
bioautography A method for detecting a trace amount of a substance (e.g. a vitamin) in a complex mixture, the given substance
being an essential growth requirement for the test organism used.
The components of the mixture are initially separated by CHROMATOGRAPHY. The presence of a given substance, in a given
chromatographic band, is then determined by extracting the band
with an appropriate solvent and adding the extract to a medium
which lacks a particular growth factor; the medium is then inoculated with an organism which fails to grow in the absence of
the growth factor. On incubation, growth of the test organism
indicates the presence of the growth requirement in the original
mixture. (cf. BIOASSAY.)
Biobor An organoboron preservative used e.g. in various liquid
hydrocarbon fuels.
bioburden In an industrial sterilization process: the number of
contaminating organisms per product unit before sterilization.
biochemical oxygen demand See BOD.
biocide (1) Syn. STERILANT. (2) Sometimes used to refer to a
DISINFECTANT or PRESERVATIVE.
bioconcentration factor See BCF.
biocontrol Syn. BIOLOGICAL CONTROL.
bioconversion (1) The conversion of a substrate to particular
product(s) by cells or by isolated enzymes. (2) The conversion
of substrate(s) to cell biomass.
biocytin e-N-Biotinyl-lysine (see BIOTIN).
biodegradation The degradation of a substance as a result
of biological (usually microbial) activity. In ecological terms,
biodegradation is vital for the recycling of matter (see e.g. CARBON CYCLE). In human terms, biodegradation may be useful e.g.
in the disposal of waste materials (see e.g. SEWAGE TREATMENT)
and xenobiotics (see BIOREMEDIATION), and in processes such as
COFFEE production and RETTING; it can also be a nuisance see
BIODETERIORATION.
biodeterioration The deterioration (spoilage) of an object or
material as a result of biological usually microbial activity.
See e.g. CATHODIC DEPOLARIZATION THEORY (of iron corrosion),
COAL BIODEGRADATION, FOOD SPOILAGE, GLASS, LEATHER SPOILAGE,
PAINT SPOILAGE, PAPER SPOILAGE, PETROLEUM (spoilage of fuels
and oils), RUBBER SPOILAGE, TEXTILE SPOILAGE, TIMBER SPOILAGE,
WOOL SPOILAGE. (See also PRESERVATIVES; cf. BIODEGRADATION.)
bioemulsifiers See BIOSURFACTANTS.
biofilm An adherent layer of microbial cells embedded in a
polymer matrix secreted by the cells. Biofilms can develop
on living tissues (e.g. oral cavity) on catheters, in water pipes
[FEMS Ecol. (1997) 22 265279], and on ships hulls; pathogens
in biofilms (e.g. on prostheses) may be resistant to antibiotics
(and to the immune system), but biofilms can be useful e.g.
in waste-water treatment systems [TIBtech.(2000) 18 312320].
(See also EPILITHON.)
95
bioreactor
All bioluminescent organisms contain a species-specific thiolcontaining oxidoreductase which catalyses oxidation of the
light-emitting entity giving rise to an energized form which
produces light as it returns to the unexcited ground state.
The generic term for this oxidoreductase is luciferase. In
Photobacterium fischeri, luciferase (EC 1.14.14.3) is a protein of
MWt 80000. (The firefly luciferase (EC 1.13.12.7) is a protein
of MWt 62000.)
Bioluminescence in bacteria. The luminescent bacteria include
marine and coastal species, e.g. Alteromonas hanedai and
species of PHOTOBACTERIUM and XENORHABDUS. All the luminescent bacteria appear to generate light by similar reactions,
involving the same types of component, and light is emitted
continuously (i.e. not in pulses) under appropriate conditions.
Bacterial luciferase is an AUTOINDUCIBLE ENZYME. The autoinducer in e.g. P. fischeri is N-(b-ketocaproyl)homoserine lactone
(see QUORUM SENSING); above a certain concentration, autoinducer switches on the lux operon that encodes luciferase.
Bacterial bioluminescence apparently involves the initial
reduction of FMN by NADH, and the formation of a
luciferaseFMNH2 complex. In the presence of (i) free
oxygen, and (ii) an aliphatic aldehyde (containing at least
seven or eight carbon atoms), a larger complex appears to
develop: luciferaseFMNH2 O2 RCHO; this complex emits
light and yields FMN, luciferase, water and a carboxylic acid
corresponding to the aldehyde. (The aldehyde may be re-cycled
after reduction of the carboxylic acid by NADH.)
Bacterial bioluminescence competes with the respiratory chain
for reduced NAD; luminescence is rapidly enhanced following
the inhibition of respiration by cyanide.
Bioluminescence in fungi. The fruiting bodies and/or mycelium
of some agarics (e.g. Armillaria mellea, Mycena spp) produce a
continuous (non-pulsing) light which, in some species, exhibits
a diurnal fluctuation in intensity; it is dependent on NAD(P)H
and appears to involve two types of enzyme. The emitted light
may be bluish-green or green (wavelength ca. 530 nm).
Bioluminescence in dinoflagellates. On appropriate stimulation (e.g. acidification, agitation), the cells of some dinoflagellates (e.g. species of Gonyaulax, Noctiluca, Pyrocystis,
Pyrodinium) emit bluish light (wavelength ca. 480 nm) in flashes
of ca. 0.1 second duration. Gonyaulax has a system of subcellular, guanine-containing, crystal-like fluorescent structures
referred to as scintillons; the luciferin occurs (together with
at least some luciferase) only in the scintillons, although some
luciferase may also occur in other parts of the cell [JCB (1985)
100 14351446]. Structures similar to scintillons have been
observed in non-luminescent dinoflagellates. Bioluminescence
in G. polyedra (and probably in many other dinoflagellates)
exhibits a CIRCADIAN RHYTHM. In Noctiluca, luminescence is
associated with subcellular organelles, the microsources.
Bioluminescence is also exhibited by a number of radiolarians.
The function of microbial bioluminescence, if any, is
unknown. It has been suggested that it is the vestige of a system
once used for removing low levels of environmental oxygen.
Applications. Bioluminescent bacteria have been used for
detecting very low concentrations of dissolved oxygen.
The ATP-dependent firefly luciferaseluciferin system is used
for detecting/quantifying ATP (e.g. in PYROSEQUENCING, in which
pyrophosphate is first converted to ATP). A luciferase reporter
system is used e.g. for studying promoter function [AEM (2005)
71 13561363] and the efficacy of antisense oligomers [AAC
(2005) 49 249255]. Three different luciferases have monitored
the simultaneous expression of three genes [BioTechniques
(2005) 38 891894].
biomass The dry weight, or other (usually quantitative) estimation of organisms (commonly microorganisms), in a given
habitat (soil, water, culture medium, etc).
biomimetic technology Biologically-based systems which can
achieve results similar to those hitherto dependent on abiotic electrical/mechanical/chemical methodology. One example
involves the ability of a strain of Pseudomonas stutzeri to form
(in its periplasm) crystalline particles of silver in a nanometre
range of sizes; heat treatment (400 C) of a layer of particlecontaining cells can form a carbonaceous matrix containing the
small, homogeneously embedded particles of silver a structure
which may have applications as a coating for the absorption of
solar energy. Silvercarbon films from P. stutzeri may also be
useful (as a consequence of their high porosity) as electrodes in
lithium-ion and other batteries.
In general, certain microorganisms are capable of producing
intracellular or extracellular cermet (ceramicmetal) or orgmet
(organicmetal) structures, or composites, which are organized
on a nanometre scale and which potentially have a range of
applications in materials science.
[Metal-accumulating bacteria and their potential for materials
science: TIBtech. (2001) 19 1520.]
biomineralization The deposition of minerals due to biological
activity e.g. the formation of magnetosomes (see MAGNETOTACTIC BACTERIA) and the intracellular or extracellular deposition of
sulphur by photosynthetic bacteria. (cf. MINERALIZATION.)
biomining See LEACHING.
Biomyxa See GRANULORETICULOSEA.
biont Syn. SYMBIONT.
biopesticide See BIOLOGICAL CONTROL.
biophore A host cell in genetic engineering.
bioplastics See BIOPOL.
Biopol The trade name (Zeneca, Great Britain) for a
range of biodegradable thermoplastics based on POLY-bHYDROXYBUTYRATE (PHB). The homopolymer (PHB) is formed
under suitable conditions when Alcaligenes eutrophus uses
glucose as the sole source of carbon. When the growth medium
is appropriately supplemented, A. eutrophus forms co-polymers
of hydroxybutyrate and hydroxyvalerate; the proportion of
hydroxyvalerate (controlled by adjusting the growth medium)
determines the properties of these co-polymers. The intracellular
granules of polymer (either PHB or co-polymer) are harvested
and purified to a fine, white powder.
Biopol can be used for making containers, mouldings, fibres,
films and coatings, and can be worked by blow-moulding and
injection-moulding processes. While stable in normal use, Biopol
is fully degradable after suitable disposal.
To reduce costs, attempts are now being made to develop
transgenic plants for the commercial production of bioplastics.
[Review on bioplastics: BAB (1996) 49 114.]
biopsy (1) The removal of tissue from the living body for
examination, culture etc. (2) The tissue specimen referred to
in (1).
biopterin 2-Amino-4-hydroxy-6-(1 ,2 -dihydroxypropyl)-pteridine. Biopterin is believed to act as a coenzyme in certain
hydroxylation reactions, and is required as a growth factor e.g.
by Crithidia fasciculata and Trypanosoma platydactyli (formerly
Leishmania tarentolae); the requirement for biopterin may be
partially or totally overcome by high concentrations of FOLIC
ACID.
bioreactor (reactor) A FERMENTER or other apparatus used for BIOCONVERSIONS.
97
bioremediation
Gram-positive bacteria. Genes encoding the relevant degradative
activity for biphenyls/polychlorinated biphenyls form the bph
operon. [Transcription of the bph operon in Pseudomonas pseudoalcaligenes strain KF707: JBC (2000) 275 3101631023.]
The pesticide pentachlorophenol (PCP) can be degraded by
strains of the bacterium Sphingomonas chlorophenolica the
metabolic potential for such degradation probably having developed during the last few decades [TIBS (2000) 25 261265].
(See also POLYURETHANASE and TOL PLASMID.)
Wastewater containing terephthalic acid (used e.g. in the
manufacture of plastics) can be treated anaerobically (see
SEWAGE TREATMENT).
[Heavy metals: FEMS Reviews (2002) 26 327338.]
The development of genetically engineered bacteria for
degrading specific compounds (particularly XENOBIOTICS) is
likely to be assisted by information on the way in which signals from various environmental substrates are integrated at gene
promoters [EMBO (2001) 20 111].
Bios test A test used for assessing the integrity of the seams
in a can (see CANNING). Essentially, cans are filled with a
nutrient medium and are sealed and processed in the normal
way cooling being carried out with water containing a gasproducing organism; the cans are then incubated and examined
for the presence of SWELLS. An analogous test is used for testing
the integrity of RETORT POUCHES.
biostratigraphy The study of the age and structure of stratified rocks in terms of the fossils e.g. FOSSIL MICROORGANISMS they contain. [Book ref. 136.]
biosurfactants Biological molecules which function as surfactants, i.e., they lower the surface tension of water; however,
as commonly used, the term includes bioemulsifiers: substances
which act as emulsifying agents but which do not necessarily have a significant effect on surface tension. Most biosurfactants/bioemulsifiers are amphipathic cell components such
as fatty acids, phospholipids, lipopolysaccharides, lipoteichoic
acids, etc. Certain microorganisms produce extracellular biosurfactants or bioemulsifiers which may play a role e.g. in the
adhesion of cells to and/or their detachment from surfaces
(see e.g. EMULCYAN), or in the utilization of hydrophobic substrates such as sulphur and hydrocarbons. For example, organisms growing on HYDROCARBONS may produce extracellular fatty
acids, glycolipids (e.g. RHAMNOLIPIDS, SOPHOROLIPIDS), highMWt polymers (e.g. EMULSAN), etc (see also LIPOSAN); such
substances may serve e.g. to emulsify the substrate and/or to
allow cells to adhere to substratewater interfaces. (See also
SAPONINS and SURFACTIN.) [Potential use of biosurfactants in
industry: MS (1986) 3 145149.]
biotechnology In a broad sense: collectively, the various forms
of technology that exploit biological sources usually microorganisms and/or their products and components (for examples see
INDUSTRIAL MICROBIOLOGY). (See also BIOMIMETIC TECHNOLOGY
and IMMOBILIZATION.) However, the term biotechnology refers
more commonly to those forms of technology which depend
on the use of modern techniques in molecular biology/genetic
engineering to construct novel organisms and/or products for
industrial, medical or other purposes.
bioterrorism See BIOLOGICAL WARFARE.
biotic Living; of biological origin.
biotin (vitamin H; coenzyme R) A VITAMIN which acts as a
cofactor in carboxylation and transcarboxylation reactions, acting as a carrier of CO2 ; biotin is bound via its carboxyl group
(see figure) to the e-amino group of a lysine residue in the apoenzyme. (cf. BIOCYTIN.)
black beans
HN1
4
5
3NH
NH
3
1
(a)
or S (dihydroxydiphenylsulphides). For maximum antimicrobial activity, each phenolic residue must carry an o(2-)hydroxyl. Halogenation increases activity; two di- or trihalogenated phenolic groups generally confer greater activity
against Gram-positive than Gram-negative species. Bacteriostatic at low concentrations, bisphenols may be bactericidal
at higher concentrations; they appear to affect the cell membrane e.g. hexachlorophane affects membrane potentials and,
at higher concentrations, may (like various antibacterial agents)
cause coagulation of the cytoplasm.
Bisphenols are poorly soluble or virtually insoluble in
water but are soluble in dilute alkali and/or organic solvents;
they are inactivated by non-ionic surfactants. Since bisphenols
retain antimicrobial activity in the presence of soaps and
are relatively non-toxic to man, they are widely used
as antiseptics and preservatives. Bithionol (2,2 -dihydroxy3,5,3 ,5 -tetrachlorodiphenylsulphide) is an antibacterial and
antifungal agent used e.g. in antiseptic soaps. Bromochlorophane
(3,3 -dibromo-5,5 -dichloro-2,2 -dihydroxydiphenylmethane) is
active against Gram-positive bacteria and has been used e.g.
in deodorants and toothpastes. Dichlorophane (dichlorophene)
(5,5 -dichloro-2,2 -dihydroxydiphenylmethane) is active against
fungi, bacteria and algae; it is used e.g. as a preservative
for paper and textiles. Fentichlor (2,2 -dihydroxy-5,5 dichlorodiphenylsulphide) is active primarily against Grampositive bacteria (e.g. staphylococci) and fungi (particularly
dermatophytes); it has been used to treat infections involving
dermatophytes. Hexachlorophane (hexachlorophene) (2,2 dihydroxy-3,5,6,3 ,5 ,6 -hexachlorodiphenylmethane) is much
more active against Gram-positive than Gram-negative bacteria;
it has been used in antiseptic soaps, liquid soaps (e.g. Ster-zac)
and lotions (e.g. pHisoHex ). (cf. TRICLOSAN; see also PHENOLS.)
bisterigmate Having two sterigmata.
bis(tri-n-butyltin) oxide See TBTO.
bisulphite (as a MUTAGEN) Bisulphite (HSO3 ) undergoes various reactions with nucleic acids, and can also cause cross-linking
between proteins and nucleic acids. The reaction believed to be
responsible for mutagenesis is the deamination of cytosine and
(at a slower rate) of 5-methylcytosine to give, respectively, uracil
and thymine (resulting in GC-to-AT transition in either case);
bisulphite can apparently act on these bases only in ssDNA. (See
also SITE-SPECIFIC MUTAGENESIS.)
bithionol See BISPHENOLS.
Bittner virus Syn. MOUSE MAMMARY TUMOUR VIRUS.
bitty cream See MILK SPOILAGE.
bitunicate ascus (fissitunicate ascus) An ASCUS whose wall consists of a thin, more or less rigid outer envelope (ectotunica),
and a thicker, extensible inner envelope (endotunica); at maturity, the outer envelope ruptures and the inner envelope elongates the ascospores being discharged via an apical pore in
the inner envelope. (cf. UNITUNICATE ASCUS.) Lecanoralean asci
release their ascospores in a similar way; they differ from other
bitunicate asci e.g. in that the endotunica protrudes only to a
limited extent during ascospore discharge.
biuret test A test based on the fact that peptide bond-containing
substances (e.g. peptides and proteins) give a violet/pink colour
when treated with a dilute, alkaline solution of copper sulphate.
bivalent (noun) See MEIOSIS.
Bivalvulida See MYXOSPOREA.
BK virus See POLYOMAVIRUS.
BL-type starter See LACTIC ACID STARTERS.
bla gene A gene encoding b-LACTAMASE. (See also e.g. Tn3.)
black beans Syn. HAMANATTO.
O
O C
(CH2)4
COOH
(b)
(CH2)4
C O
N H
protein
bleeding canker
present in large numbers [Ped. Inf. Dis. (1985) 4 556557].
Three morphological forms (amoebic, granular and vacuolated)
have been described, but the vacuolated form is the most common in human faecal specimens; these cells are non-motile and
spherical, oval or ellipsoid, (5)810(30) m diam., and may
be mistaken for cysts of certain amoebae. Staining of the vacuolated forms with e.g. iodine reveals a thin peripheral layer of
cytoplasm containing one nucleus (sometimes 24 nuclei) and
surrounding a large central or slightly eccentric body or vacuole.
Blastodinium See DINOFLAGELLATES.
Blastomyces A genus of fungi of the HYPHOMYCETES. B. dermatitidis (= B. zymonema, teleomorph Ajellomyces dermatitidis) is a
dimorphic fungus which causes BLASTOMYCOSIS; in mammalian
cells and in culture at 37 C it grows in the form of yeast-like,
spherical, thick-walled cells (usually ca. 815 m diam.). The
cells reproduce by budding, a (usually) single bud being attached
to the mother cell by a broad base. When cultured at <30 C
the organism grows as a septate mycelium, producing smooth,
spherical to ovoid conidia (35 m diam.) on short, straight
conidiophores.
Blastomycetes A class of fungi (subdivision DEUTEROMYCOTINA)
which include the anamorphic yeasts; the class is sometimes
divided into two families: CRYPTOCOCCACEAE (species do not
form ballistospores) and SPOROBOLOMYCETACEAE (species form
ballistospores). In some taxonomic schemes [Book ref. 64,
p. 54] the organisms are included in the HYPHOMYCETES.
blastomycosis (North American blastomycosis; Gilchrists disease) An acute or chronic MYCOSIS, affecting man and animals (e.g. dogs), caused by Blastomyces dermatitidis; it occurs
e.g. in North America, Africa and Israel. Infection apparently
occurs by inhalation of spores from the (presumably saprotrophic) fungus, although B. dermatitidis has proved difficult
to isolate from environmental habitats. The disease occurs in
two clinically distinct but variable forms: the cutaneous form
(a chronic disease in which granulomatous, suppurative lesions
are confined mainly to the skin, although the pathogen is disseminated from a primary pulmonary site), and the pulmonary
form (in which lesions develop primarily in the lungs). Pulmonary blastomycosis may be subclinical, may (occasionally)
manifest as an acute, self-limiting, influenza- or pneumonia-like
disease, or may be chronic and progressive with dissemination
to other regions of the body (e.g. bones, genitourinary tract,
CNS). Mortality rates associated with untreated systemic blastomycosis may be >80%. Chemotherapy: e.g. amphotericin B;
2-hydroxystilbamidine. [Review of human blastomycosis: CRM
(1982) 9 139164.] (cf. PARACOCCIDIOIDOMYCOSIS.)
blastospore See CONIDIUM.
Blattabacterium A genus of Gram negative-type bacteria which
occur as intracellular endosymbionts of the cockroach (Blatta
spp). Cells: non-motile rods, ca. 1.0 1.69.0 m, which may
give a Gram-positive or Gram-variable reaction; they occur
within the bacteriocytes of the cockroach and within the
oocytes, thus ensuring their transmission to the larvae. GC%: ca.
2628. Type species: B. cuenoti. [Book ref. 22, pp. 830831.]
bleach See HYPOCHLORITES.
bleaching Loss of the chromophore from a biological pigment,
or loss of pigment(s) from an organism e.g. loss of chlorophyll
from a photosynthetic organism.
bleeding canker A CANKER which affects e.g. horse chestnut,
lime and apple trees; it is caused by Phytophthora citricola. A
brownish or reddish gum oozes from the regions of dying bark
and dries to form a hard black crust; dieback may occur, and
the lesions may be infected with other wood-decaying fungi.
blending
combine with allergens and which prevent those allergens from
initiating an immediate hypersensitivity reaction.
blood agar An agar-based medium containing defibrinated (or
whole citrated or oxalated) blood. It is prepared by mixing
510% blood (drawn aseptically) with a pre-autoclaved molten
agar base (e.g. TRYPTICASESOY AGAR) at ca. 50 C; the medium is
dispensed e.g. to Petri dishes and allowed to set. (cf. CHOCOLATE
AGAR.) Blood agar is used e.g. for the culture of fastidious
bacterial parasites of man and animals, and for the detection of
HAEMOLYSINS; since a given bacterial haemolysin may be active
against the RBCs of only some animals (e.g. horse, sheep), the
choice of blood is important.
blood clotting See FIBRIN; COAGULASE; ANTICOAGULANT.
blood culture A procedure for detecting the presence of viable
bacteria in blood. Since blood-borne bacteria may be present
only in very small numbers, isolation is attempted only after
a blood sample has been incubated in a suitable medium
to allow the bacteria to multiply. Blood (510 ml), taken
aseptically, is immediately added (aseptically) to 50100 ml
of medium (e.g. trypticase soy broth) which usually contains
an anticoagulant (e.g. SPS) and sometimes e.g. penicillinase
(to inactivate any penicillin in the blood) and/or PABA (to
counteract any sulphonamide drugs). (The medium is commonly
contained in a plain bottle whose opening is sealed by a rubber
disc held in place by a screw-cap with a central hole; blood is
injected into the bottle through the rubber disc.) The medium is
then incubated. Periodically (e.g. daily for 7 days) the medium is
subcultured to a suitable solid medium which is then incubated
blunt-ended DNA
blue bodies See EAST COAST FEVER.
blue cheese See CHEESE-MAKING.
blue-eared pig disease Porcine reproductive and respiratory syndrome (PRRS): a disease of pigs, reported first in the USA and
later in Europe, associated with a variety of symptoms, including abortion/stillbirth, agalactia, respiratory distress (particularly
in new-born animals) and cyanosis of the ears; some strains can
cause encephalitis. The disease may be mild, or may be severe
with heavy losses, depending e.g. on the virulence of the causal
agent and existing health of infected pigs. Secondary infections
may occur.
The causal agent is a virus (genus ARTERIVIRUS), first identified
in The Netherlands (the Lelystad virus); it is also referred to
as the swine infertility and respiratory syndrome (SIRS) virus.
Infection may occur via the airborne route. The incubation
period may be a few days to a week, or much longer. Following
experimental infection via the oronasal route, the virus can
be detected within 12 hours in alveolar macrophages, in lung
lymph nodes within 24 hours, and in spleen within 34 days. A
reduction in numbers of alveolar macrophages (the major target
cell of the virus) may be important in predisposing to secondary
infections. Virus is shed in the oronasal secretions, urine and
faeces of acutely infected animals.
[PRRS: RMM (1995) 6 119125.]
blue-green algae CYANOBACTERIA.
blue-light fluorescence See FLUORESCENCE.
blue mould (1) (of tobacco) See PERONOSPORA.
(2) Any blue-spored species of Penicillium.
blue proteins Copper-containing proteins which characteristically absorb strongly at or near 600 nm; at least some blue
proteins are known to have roles in electron transport, and these
proteins have been referred to as cupredoxins.
Blue proteins occur in bacteria, e.g. AMICYANIN, AZURIN
(sense 1), RUSTICYANIN; in fungi, e.g. LACCASE; in higher plants,
e.g. cucumber basic blue protein, stellacyanin, umecyanin; in
higher plants, algae and cyanobacteria, e.g. PLASTOCYANIN; and in
animals, e.g. ascorbate oxidase (EC 1.10.3.3) and ceruloplasmin
(found in mammalian blood plasma).
blue pus Pus formed in suppurative infections involving Pseudomonas aeruginosa; the pus has a bluish tinge owing to the
presence of pyocyanin.
blue slime disease See COSTIASIS.
blue-stain A form of SAP-STAIN in which timber becomes bluishgrey owing to the deep penetration of fungal hyphae; the
bluish-grey stain is due to refraction of light by the hyphae.
The commonest causal agents of blue-stain in temperate zones
are species of Ceratocystis, e.g. C. pilifera; Diplodia spp are
important in the tropics. Blue-stain may reduce the value of
timber, but it does not significantly affect its mechanical strength
since the cellulose and lignin components of the wood are little
affected.
blueberry shoestring virus See SOBEMOVIRUSES.
bluecomb disease virus See CORONAVIRIDAE.
bluetongue An acute SHEEP DISEASE caused by an ORBIVIRUS;
other ruminants (e.g. cattle, deer) may be affected, but in these
the disease is usually mild or subclinical. Bluetongue occurs
mainly in Africa but has occurred e.g. in Europe, Asia, USA.
Transmission occurs mainly via a biological vector (especially
Culicoides spp). Incubation period: 2 days to 2 weeks. Symptoms: fever; inflammation and cyanosis of the mucous membranes of the mouth, nose, and alimentary tract. The lungs and
feet may be involved. Mortality (in sheep): e.g. 530%.
blunt-ended DNA Linear dsDNA with flush ends, i.e., with no
3 or 5 single-stranded extensions. (cf. e.g. STICKY ENDS.)
blusher
blusher Amanita rubescens.
BLV Bovine leukosis virus: see BOVINE VIRAL LEUKOSIS.
BOD (biochemical oxygen demand; biological oxygen demand)
The amount of dissolved oxygen needed for microbial oxidation
of soluble, biodegradable matter in an aquatic environment. For
example, when discharged to rivers etc., sewage effluents may
consume large amounts of dissolved oxygen, and if dilution
is inadequate they may give rise, locally, to anaerobic or
microaerobic conditions (i.e. exert a high BOD); in such cases
there is a risk of asphyxiation for fish and other organisms
dependent on appropriate levels of dissolved oxygen.
The BOD test measures the amount of oxygen (mg) consumed
per litre of (e.g.) sewage, or a known dilution of it, in 5 days
at 20 C.
(See also SEWAGE TREATMENT.)
BOD test See BOD.
Bodanella See PHAEOPHYTA.
Bodo A genus of protozoa (suborder BODONINA); species occur
e.g. in organically polluted waters (see SAPROBITY SYSTEM). The
cells are ovoid or tapered, sometimes flattened, ca. 520 m in
length; two flagella arise at the anterior end (near the cytostome),
one being directed posteriorly.
Bodonina A suborder of biflagellate protozoa (order KINETOPLASTIDA); some members are free-living, others are parasitic e.g.
in the blood or gut of fish. Genera include BODO, Cryptobia,
Rhynchomonas.
body microflora Each of the various regions of the body
typically harbours a characteristic MICROFLORA (sense 1); for
microflora of the human body see e.g. EAR MICROFLORA,
EYE MICROFLORA, GASTROINTESTINAL TRACT FLORA, GENITOURINARY TRACT FLORA, MOUTH MICROFLORA, RESPIRATORY TRACT
MICROFLORA, SKIN MICROFLORA.
body odour See SKIN MICROFLORA.
boil (furuncle) A skin lesion due to infection of a hair follicle,
sebaceous gland or skin lesion by (usually) Staphylococcus
aureus. A tender red nodule becomes pus-filled and may either
subside or break at the skin surface and drain. (cf. CARBUNCLE;
FURUNCULOSIS (2).)
boil disease (in fish) See MYXOBOLUS.
Boivin antigens Syn. O ANTIGENS.
Bolbitiaceae See AGARICALES.
Boletales An order of fungi (subclass HOLOBASIDIOMYCETIDAE)
that typically form mushroom-shaped basidiocarps in which
the hymenophore lines a mass of vertically orientated tubules
on the underside of the pileus (porous basidiocarp) or forms
a layer on lamellae; the porous basidiocarps are fleshy (cf.
APHYLLOPHORALES). Genera include e.g. Boletus (basidiocarp
porous, stipe central), Paxillus (lamellate), and Phylloporus
(lamellate). Some species are edible e.g. Boletus edulis (c`epe
or penny bun), some form mycorrhizal associations with trees,
and one species, Boletus parasiticus, is parasitic on Scleroderma.
[Classification and spore structure: TBMS (1981) 76 103146.]
Boletus See BOLETALES.
Boletus virus See POTEXVIRUSES.
Bolivian haemorrhagic fever A VIRAL HAEMORRHAGIC FEVER
caused by the Machupo virus (see ARENAVIRIDAE). Mortality:
usually ca. 530%.
Bombyx mori NPV See NUCLEAR POLYHEDROSIS VIRUSES.
bongkrek See TEMPEH.
bongkrekic acid A toxic, substituted heptaenedioic acid produced by Pseudomonas cocovenenans in spoiled bongkrek (see
TEMPEH); it inhibits (uncompetitively) the ADP/ATP exchange
carrier system which operates across the inner mitochondrial
membrane. (cf. ATRACTYLOSIDE.)
botulinum toxin
botches disease Synonym for freshwater RED PEST.
bothrosome See LABYRINTHULAS and THRAUSTOCHYTRIDS.
boticins See BACTERIOCIN.
Botrydium
A genus of siphonaceous algae (class XANTHOPHYCEAE) in which the mature vegetative organism consists of a
globose to elongate (typically pear-shaped) coenocytic vesicle,
up to ca. 2 mm diam., anchored to the substratum (mud, damp
soil, etc) by colourless branched rhizoids; inside the vesicle is
a thin peripheral layer of cytoplasm (containing the chloroplasts
and nuclei) surrounding a large central vacuole. Asexual reproduction occurs by the formation of zoospores or aplanospores;
resistant cysts are formed under dry conditions.
Botryobasidium See APHYLLOPHORALES (Corticiaceae).
botryomycosis (bacterial pseudomycosis) A chronic localized
infection of the skin and subcutaneous tissues in man
and animals. The pathogen (commonly e.g. Pseudomonas
aeruginosa, Staphylococcus aureus, or Escherichia coli ) forms
one or more granules in the centre of an abscess which is
surrounded by fibrous tissue. (cf. MADUROMYCOSIS.)
Botryotinia See HELOTIALES.
botrytis (plant pathol.) Syn. GREY MOULD.
Botrytis A genus of fungi of the class HYPHOMYCETES; many
species are known to have teleomorphs in the genus Botryotinia.
The organisms include many plant-pathogenic species e.g.
B. aclada (= B. allii ) (see ONION ROT), B. cinerea (see GREY
MOULD, NOBLE ROT), and B. fabae (see CHOCOLATE SPOT). (See
also SOFT ROT sense 2.) Antifungal agents used against Botrytis
infections include e.g. BENOMYL, DICARBOXIMIDES, DICHLOFLUANID, DICLORAN, THIRAM and ZINEB.
Botrytis spp form septate mycelium; dark, ovoid, non-septate
conidia develop in a layer on the swollen, terminal region of each
of the small branches of a conidiophore. Sclerotia are formed e.g.
by B. aclada, B. cinerea and B. tulipae. [Book ref. 183.]
bottom-fermenting yeast See BREWING.
bottromycins A group of peptide antibiotics, produced by Streptomyces spp, which inhibit bacterial protein synthesis.
botulinolysin See THIOL-ACTIVATED CYTOLYSINS. (cf. BOTULINUM
TOXIN.)
botulinum C2 toxin A powerful toxin, produced by certain
strains of Clostridium botulinum, which apparently has no
neurotoxic activity (cf. BOTULINUM TOXIN) but which causes
e.g. increased intestinal secretion. The C2 toxin consists of two
components, the larger of which appears to be involved in cellsurface binding and (possibly) uptake of the smaller component.
The smaller component effects ADP-RIBOSYLATION of an ATPbinding ACTIN molecule, G actin, preventing its polymerization
to F actin; this disrupts the cells microfilament cytoskeleton and
leads e.g. to rounding of the cell.
botulinum cook In the food processing industry: COOKING equivalent to a 12D PROCESS in respect of the endospores of Clostridium botulinum. The D121.1 value (see D VALUE) of C. botulinum
endospores is generally taken to be ca. 0.21 min. (See also CANNING.)
botulinum toxin Any of a range of related, powerful protein toxins (MWt ca. 150000) produced mainly by strains of Clostridium
botulinum.
Botulinum toxins are differentiated antigenically into types
AG, with type C being divided into subtypes C1 and C2. Toxins
of types AF with the exception of BOTULINUM C2 TOXIN are
powerful neurotoxins which cause BOTULISM in man and animals.
The (plasmid-encoded) botulinum toxin G has been isolated e.g.
from autopsy material but has not been linked definitively with
disease. The botulinum C and D toxins are encoded by genes
from two different bacteriophages.
botulism
Wound botulism is a rare form of the disease resulting from
contamination of a wound by a toxigenic strain of the pathogen.
Incubation period 414 days. Symptoms are similar to those
of food-borne botulism, sometimes with the addition of fever.
Infant botulism can follow ingestion of spores of the pathogen
which germinate and form toxin in the gut (= toxicoinfection).
The disease affects mainly infants <6 months of age, and
varies from subclinical to rapidly fatal; typical symptoms: e.g.
constipation, lethargy, dysphagia and weakness. One source
of infection was reported to be honey contaminated with
C. botulinum spores [JPed (1979) 94 331338]. Infant botulism
may be responsible for some cases of SUDDEN INFANT DEATH
SYNDROME; sudden death may be due to weakening or flaccid
paralysis of muscles of the tongue and pharynx, leading to
obstruction of the airway and asphyxia.
Botulism of undetermined classification includes those cases
in individuals, older than 1 year, in which a specific food cause
cannot be implicated. Botulism in an adult may be due to the
synthesis of toxin within the intestine during a gut infection
with the pathogen [NEJM (1986) 315 239241; Lancet (1987)
i 357360; (C. barati ) JCM (2002) 40 22602262].
Lab. diagnosis (all forms): assay of serum, faeces and
implicated foods for botulinum toxin and organisms.
Treatment. Any unabsorbed toxin should be removed from
the gut. Polyvalent antitoxin may be administered (avoiding
possible hypersensitivity reactions to heterologous components).
Guanidine, given orally, may counteract the effects of toxin
at the nervemuscle junction. Supportive care will be needed.
(A prophylactic botulinum toxoid vaccine has been given to
laboratory personnel working with C. botulinum, but such a
vaccine is unlikely to be useful for treatment owing to the time
required to develop an immune response.)
[Botulism (epidemiology, diagnosis, treatment): RMM (1995)
6 5862.]
(b) Botulism in animals. In cattle, the disease may be caused
by C. botulinum types B, C or D (see e.g. LAMZIEKTE and
MIDLAND CATTLE DISEASE). In horses, types B or C may be
involved (see e.g. FORAGE POISONING). Birds may be affected by
types A or C (see e.g. LIMBERNECK and WESTERN DUCK DISEASE).
In farmed salmonid fish the disease has been caused by type
E [J. Fish Dis. (1982) 5 393399]. In animals, the disease is
characterized by progressive paralysis without loss of sensibility
and without fever.
Boucherie process A method of TIMBER PRESERVATION in which
the sap of newly felled trees is replaced by a preservative (under
pressure) in order to prevent subsequent fungal decay of the
timber. (cf. SAUGKAPPE PROCESS; BETHELL PROCESS.)
Bouins fluid A FIXATIVE: a mixture of picric acid (75 ml
saturated, aqueous), formalin (25 ml), and glacial acetic acid
(5 ml).
bound coagulase See COAGULASE.
bourbon See SPIRITS.
boutonneuse In man: a mild disease caused by Rickettsia conorii
and transmitted by tick bite. After an incubation period of 12
weeks a characteristic lesion (the tache noir ) develops at the
location of the bite; this lesion (up to 0.5 cm diam.) consists
of a black necrotic centre and a reddened margin. The regional
lymph nodes may be affected. Fever, headache and muscular
pains are typically followed by a maculopapular rash. Diagnosis
may include the WEILFELIX TEST.
Boveria See SCUTICOCILIATIDA.
Boverin See BEAUVERIA.
bovid herpesvirus See under bovine herpesvirus.
Boyden procedure
BSE prion converts human PrP to the prion form in a cell-free
system [Nature (1997) 388 285288]. [Review of BSE: RMM
(1998) 9 119127.]
[Cumulative incidence of BSE in the United Kingdom during
the period July 1986June 1997, animal-associated risk factors
influencing age of onset of clinical signs, and effectiveness of
control measures: VR (2000) 147 349354.]
(See also CATTLE DISEASES.)
bovine syncytial virus See SPUMAVIRINAE.
bovine tubercle bacillus Mycobacterium bovis.
bovine typhus Syn. RINDERPEST.
bovine ulcerative mammillitis (bovine herpes mammillitis) A
CATTLE DISEASE caused by bovine (alpha) herpesvirus 2 (bovine
mammillitis virus see ALPHAHERPESVIRINAE). The disease
involves severe inflammation and ulceration of the skin of
the udder and teats; stomatitis and facial infection may also
occur, particularly in calves. (See also LUMPY SKIN DISEASE and
MASTITIS.)
bovine viral leukosis (enzootic bovine leukaemia) A chronic
transmissible CATTLE DISEASE caused by the bovine leukosis virus
(BLV), an exogenous v-onc retrovirus which is closely related
to HTLV-I and HTLV-II (see HTLV). [Nucleotide sequence of the
BVL genome and its relation to other retroviruses: PNAS (1985)
82 677681.] Natural infection occurs e.g. in cattle (Bos taurus
and Bos indicus), sheep, and water buffalo. The disease involves
systemic malignant neoplasia of the reticuloendothelial system;
in a small proportion of infected animals, malignant lymphomas
(mainly of the B cell type) may develop in almost any organ,
resulting in a variety of clinical manifestations. Transmission
occurs horizontally by transfer of infected lymphocytes most
commonly via surgical instruments and needles (e.g. during herd
vaccinations, blood-sampling, etc); natural transmission may
occur via milk or colostrum or, in tropical countries, possibly
via insects or parasites. [Reviews: Book refs 105, pp. 229260,
and 110, pp. 197216.]
bovine virus diarrhoea (BVD) A CATTLE DISEASE caused by the
BVD-MD virus (see PESTIVIRUS). BVD may affect cattle (and
other ruminants) at any age, and follows infection by ingestion
or inhalation; the condition is usually mild and self-limiting. (cf.
MUCOSAL DISEASE.)
Bovista See LYCOPERDALES.
bowel oedema Syn. OEDEMA DISEASE.
BowieDick test A test used to monitor the performance of an
AUTOCLAVE. Essentially, two pieces of AUTOCLAVE TAPE are fixed
in the form of an X to a piece of paper which is inserted into
the middle of a stack of cotton towels; the towels are autoclaved
and the tape is examined. A satisfactory sterilizing regime is
deemed to have been achieved only if all parts of the tape
indicate exposure to sterilizing conditions.
box-like bacteria Variously shaped, angular bacteria which
are found in hypersaline environments and which contain
bacteriorhodopsin-like pigments [JB (1982) 151 15321542].
(cf. SQUARE BACTERIA.)
Boyden chamber A chamber, divided into two sections by a
membrane filter, used e.g. to study macrophage migration; the
filter initially separates activated T lymphocytes (or their supernatant) and macrophages the latter subsequently migrating
through the filter in response to macrophage chemotactic factor.
Boyden procedure Treatment of erythrocytes with tannic acid
(see TANNINS) to enable them to adsorb soluble antigens; such
tanned cells are used e.g. in PASSIVE AGGLUTINATION. (Chromium
salts or e.g. bis-diazobenzidine have been used in place of tannic
acid.)
bp
brain fungus Sparassis crispa.
brainheart infusion medium A medium containing infusions
of calf-brain and beef-heart, proteose, D-glucose, NaCl, and
Na2 HPO4 ; it is available commercially in dehydrated form. The
medium may be used as a broth or solidified with agar; it may
be supplemented with e.g. haemin, menadione, yeast extract etc.
It is used for the culture of a range of bacteria and medically
important fungi. [Recipe: Book ref. 47, pp. 644645.]
branch migration (mol. biol.) See RECOMBINATION (figures 1 and
2).
branched DNA assay See BDNA ASSAY.
branching enzyme An enzyme which introduces branches into
a linear polysaccharide (see e.g. GLYCOGEN and Q ENZYME). (cf.
DEBRANCHING ENZYMES.)
Branchiomyces
A genus of fungi of uncertain taxonomic
affinity; strains of Branchiomyces have features in common with
members of the SAPROLEGNIALES, but it is unknown whether they
form heterokont zoospores or aplanospores [Book ref. 1, pp.
215216]. The organisms have been isolated only from the gill
tissues of fish (see GILL ROT).
branchiomycosis Syn. GILL ROT.
brand spores See USTILAGINALES.
Brandenfleckenkrankheit Syn. BURNED SPOT DISEASE.
brandy See SPIRITS.
Branhamella See MORAXELLA.
brassica black rot See BLACK ROT.
brassica diseases See CRUCIFER DISEASES.
Braun lipoprotein (murein lipoprotein) A small lipoprotein
(MWt ca. 7500) which occurs e.g. in Escherichia coli (encoded
by gene lpp) and in other enterobacteria; each cell contains ca.
105 106 copies of the lipoprotein about one-third of which
form links (in association with OmpA) between the peptidoglycan layer and the OUTER MEMBRANE (thus stabilizing the cell
envelope).
Braun lipoprotein is synthesized as a precursor with a signal
sequence (see SIGNAL HYPOTHESIS). The cysteine residue immediately adjacent to the signal peptide cleavage site is modified
by substitution with a diacylglycerol, permitting cleavage by
the signal peptidase; following cleavage, a fatty acid residue is
added to the N-terminal cysteine. Such post-translational modification apparently targets the protein to the outer membrane.
[Cell (1990) 61 739741.]
The activity of the signal peptidase is inhibited by the
peptide antibiotic globomycin (a structural analogue of the
cleavage site).
Braun MSK tissue disintegrator An apparatus for CELL DISRUPTION. The sample, together with glass or plastic beads, is placed
in a cooled container which is shaken at several thousand oscillations per minute for ca. 5 minutes; cells are broken by shear
forces. The apparatus can break e.g. Gram-positive bacteria and
endospores.
braxy (bradsot) An acute, usually fatal disease of lambs and
young sheep; symptoms: fever, anorexia, inflammation of the
wall of the abomasum, and toxaemia. Braxy occurs only in
winter and appears to be due to the invasion of the abomasum
by Clostridium septicum the ingestion of frozen grass being a
possible predisposing factor. Death occurs within hours.
BRD BOVINE RESPIRATORY DISEASE.
BrdU Syn. BUDR.
bread-making Bread is prepared by mixing flour (usually wheat
flour), water, BAKERS YEAST and salt to form a dough; other
ingredients (e.g. milk, sugar, shortening etc) may be added.
After thorough mixing the dough is left to prove at ca. 25 C;
bp BASE PAIR.
Bph BACTERIOPHAEOPHYTIN.
bph operon See BIOREMEDIATION
BPI protein (bactericidal/permeability-increasing protein) A
component of the azurophil granules in human and rabbit NEUTROPHILs; it is bactericidal for some Gram-negative bacteria in
which it increases the permeability of the OUTER MEMBRANE but
it is not active against e.g. POLYMYXIN-resistant enteric bacteria (such as Proteus) or Gram-positive bacteria [MR (1992) 56
399]. BPI binds to LPS and can apparently neutralize endotoxicity, and it may also attenuate the inflammatory response [see
e.g. RMM (1995) 6 101108].
BPL b-PROPIOLACTONE.
BPV Bovine papilloma virus: see PAPILLOMAVIRUS.
Brabant mastitis test See CALIFORNIA MASTITIS TEST.
Brachiomonas A genus of unicellular flagellated green algae
which are closely related to CHLAMYDOMONAS. The vegetative
cells have a distinctive morphology: the posterior end is pointed,
and four backward-directed pointed projections extend laterally
from the cell body. Motile autospores are formed (the daughter
cells acquiring the distinctive adult-cell morphology before being
released).
Brachonella See HETEROTRICHIDA.
Brachyallomyces See ALLOMYCES.
Brachyarcus A proposed genus of gas-vacuolated, curved rodshaped bacteria which occur, in groups (coenobia), in microaerobic or anaerobic sulphide-containing aquatic habitats. [Book ref.
22, pp. 137138.]
Brachybasidiales An order of plant-endoparasitic fungi (subclass
HOLOBASIDIOMYCETIDAE) which form bisterigmate basidia either
in definite hymenia or in tuft-like fascicles. Brachybasidium
forms non-septate basidiospores on tufts of basidia which emerge
from the host plants stomata. Members of the other genera form
true hymenia which emerge through the hosts epidermis and
stomata and basidiospores which sometimes become septate.
In Dicellomyces, the basidiocarp is gelatinous (when fresh) and
the hymenium is of uniform thickness. In Ceraceosorus and
Proliferobasidium the basidiocarp is waxy, and the hymenium
is not of uniform thickness; Ceraceosorus forms intracellular
hyphae, Proliferobasidium forms intercellular hyphae [Mycol.
(1976) 68 640654]. (cf. EXOBASIDIALES.)
Brachybasidium See BRACHYBASIDIALES.
bracket fungi (shelf fungi) Those fungi of the APHYLLOPHORALES
(e.g. Piptoporus betulinus) whose fruiting bodies jut out like
brackets or shelves from infected trees or rotting logs etc.
bradsot Syn. BRAXY.
Bradyrhizobium A genus of Gram-negative bacteria of the RHIZOBIACEAE; strains were formerly included in the genus RHIZOBIUM as slow-growing strains (colonies 1 mm diam. in
57 days on e.g. yeast extractmannitolmineral salts agar).
Bradyrhizobium spp produce an alkaline reaction in media containing carbohydrate (e.g. mannitol) and mineral salts. Extracellular slime includes a neutral (1 2)-b-glucan. Some strains
can grow chemolithotrophically with H2 , CO2 and low levels
of O2 ; some can fix nitrogen under microaerobic conditions in
media which contain e.g. a source of fixed nitrogen. Species
induce ROOT NODULE formation in certain leguminous plants
(mostly tropical, some temperate) e.g. soybeans, cowpea, siratro, certain Lotus spp. One non-leguminous plant, Parasponia
(Ulmaceae), is also nodulated by a Bradyrhizobium strain. GC%:
6165. Type species: B. japonicum (formerly Rhizobium japonicum). [Book ref. 22, pp. 242244.]
bradyzoite Syn. CYSTOZOITE.
108
brewing
brevetoxins Polycyclic toxins produced by the dinoflagellate
Ptychodiscus brevis (see RED TIDE). Brevetoxins A, B and C
each consist of 11 contiguous ether rings; they are highly lipidsoluble and are potent neurotoxins, causing depolarization of
nerve membranes. [PAC (1986) 58 339350 (346347).]
Brevibacterium A genus of obligately aerobic, catalase-positive,
asporogenous bacteria (order ACTINOMYCETALES, wall type
III see also PEPTIDOGLYCAN) which occur e.g. on certain
cheeses. In culture the organisms initially grow as irregular,
lumpy rods, but coccoid forms predominate in the stationary phase; colonies vary from yellow to orange-red, though
some strains produce pigment only in the light. Growth occurs
at ca. 2025 C e.g. on trypticasesoy agar containing 4%
sodium chloride; metabolism is oxidative. GC%: ca. 6064.
Type species: B. linens.
Brewer jar An ANAEROBIC JAR which consists of a cylindrical
glass chamber and a flat, gas-tight lid which is secured by
means of a screw clamp. In use, the jar is filled with e.g. a
mixture of N2 (85%), CO2 (5%) and H2 (10%), and any residual
O2 is eliminated by means of an electrically-heated platinized
catalyst which is fitted inside the lid and which is separated from
the interior of the jar by a gauze safety screen. Alternatively,
the jar may be used for the evacuationreplacement method
as described for the MCINTOSH AND FILDES ANAEROBIC JAR.
Anaerobiosis within the jar is monitored e.g. with a tube
containing a METHYLENE BLUE solution.
Brewers thioglycollate medium A liquid medium (pH 7.07.2)
used e.g. for the culture of ANAEROBES; it includes e.g. glucose, tryptone, agar (ca. 0.1%), sodium thioglycollate (a poising agent see REDOX POTENTIAL), and a redox indicator dye.
[Recipe: Book ref. 53, pp. 14091410.] The medium is particularly useful for testing the sterility of products which contain
mercurial preservatives the antimicrobial activity of the latter
being neutralized by the thioglycollate.
brewers yeast Any of various strains of Saccharomyces cerevisiae used for BREWING (q.v.); bottom-fermenting strains (formerly called Saccharomyces uvarum or S. carlsbergensis: see
SACCHAROMYCES) are usually used in the manufacture of lagers,
while top-fermenting strains are usually used for ales. (Topand bottom-fermenting strains can generally be distinguished by
the ability of bottom yeasts to produce an extracellular melibiase (a-galactosidase) and thus to hydrolyse raffinose to glucose,
galactose and fructose, whereas top yeasts which do not produce melibiase hydrolyse raffinose to melibiose and fructose.)
Particular strains of yeast may be selected for particular properties (e.g. flavour production), but all brewers yeasts must be
able to ferment the sugars (particularly maltose and maltotriose)
present in wort, and must be able to tolerate the initially high
levels of solutes in wort and produce and tolerate high levels of ethanol under brewing conditions; the yeast must also be
readily separable from the fermented wort (see BREWING) and
should retain high viability for re-use in subsequent fermentations. [Selection and modification of brewers yeast strains: Food
Mic. (1984) 1 289302.]
brewing The preparation of beer or lager by the fermentation
of an aqueous extract of malted barley containing essential oils
and bitter resins of the dried female flowers (cones) of the
hop (Humulus lupulus). During malting the barley is allowed
to germinate, and the grain starch and protein are partially
degraded by endogenous enzymes. Germination is halted by
kilning: drying (e.g. to stop respiration, preserve enzymes and
substrates etc), followed by heating (e.g. to ca. 80 C). The dried
malt is ground (milled) to expose the starchy endosperm; the
during this time the yeast metabolizes sugars (released from the
flour starches by AMYLASES present in the flour) and produces
bubbles of CO2 which become trapped in an elastic complex
of flour proteins (gluten) lightening the texture of the dough.
(Fungal amylases may be added to increase the availability
of fermentable sugars (see also PROTEASES).) In addition to its
leavening (lightening) action, the yeast contributes flavour to
the product and helps to modify the gluten structure. When the
leavened dough is baked the yeast is usually killed and any
alcohol produced by fermentation evaporates.
Sourdough breads are made by using a starter consisting
of flour (usually rye) and water inoculated with dough from
a previous batch. In the starter, heterofermentative lactic acid
bacteria (Lactobacillus sanfrancisco) ferment maltose (released
from the starch by amylase action) and produce lactic and
acetic acids, ethanol and CO2 ; the pH falls to e.g. ca. 3.8. The
acid-tolerant yeast Saccharomyces exiguus, which does not use
maltose, uses other sugars (glucose, fructose etc) to leaven the
bread. The starter may then be mixed with flour, water and salt
to make a dough as with ordinary bread.
[Gluten biochemistry: Biotechnology (1995) 13 11851190.]
bread mould See BREAD SPOILAGE.
bread spoilage Bread and similar products are very susceptible to
spoilage by the growth of moulds, especially Rhizopus nigricans
(black bread mould), Neurospora sitophila (red bread mould),
and species of Penicillium and Aspergillus. Preservatives which
may be incorporated in the dough include e.g. propionates, sorbic
acid, and potassium sorbate. (See also ROPINESS; ERGOTISM.)
breakpoint chlorination See WATER SUPPLIES.
breakage-and-reunion model See RECOMBINATION.
breakbone fever Syn. DENGUE.
breaking (plant pathol.) Syn. COLOUR-BREAKING.
Breda virus An RNA virus which causes diarrhoea in young
calves; it is apparently related to the BERNE VIRUS (see TOROVIRIDAE). [Morphological study of Breda virus replication: JGV
(1986) 67 12931304.]
brefeldin A A fungal toxin which inhibits the activity of the
Golgi apparatus and which, as a consequence, can block certain
processes in various types of cell; for example, brefeldin A can
block protein secretion and inhibit the development of viruses.
Breinl strain A virulent strain of Rickettsia prowazekii ; unlike
the attenuated E strain it can be cultivated in human macrophage
cultures.
Bremia A genus of fungi (order PERONOSPORALES) which cause
DOWNY MILDEWS on members of the Compositae (e.g. B. lactucae
on lettuce). [B. lactucae lettuce interaction: Book ref. 174, pp.
116118.]
Bremiella See PERONOSPORALES.
Brettanomyces A genus of yeasts (class HYPHOMYCETES) which
form single spheroidal, cylindrical or elongated budding cells,
pseudomycelium, or branched non-septate mycelium. Growth
occurs slowly e.g. on malt agar; species may be isolated on
cycloheximide-containing malt agar. Most strains can ferment
glucose; fermentation is usually stimulated by O2 and acetoin
(Custers effect, negative Pasteur effect). Under aerobic conditions acetic acid is produced from glucose and from ethanol.
Only some species can assimilate NO3 . Species: B. abstinens,
B. anomalus, B. bruxellensis (teleomorph: Dekkera bruxellensis), B. claussenii, B. custersianus, B. custersii, B. intermedius
(teleomorph: Dekkera intermedia), B. lambicus, B. naardenensis. (B. sphaericus = Candida etchellsii; B. versatilis =
Candida versatilis.) Species occur in beers, wines (see WINE
SPOILAGE), grape must etc. [Book ref. 100, pp. 562576.]
109
brick cheese
resulting grist is made into a mash by mixing with water. Other
carbohydrate sources (adjuncts) may be added at this stage.
The mash (pH 5.25.5) is subjected to controlled (variable)
temperaturetime cycles during which starch is broken down
to fermentable sugars (glucose, maltose, maltotriose) and nonfermentable dextrins, proteins are degraded to amino acids and
peptides, and phytin is hydrolysed to inorganic phosphate (which
acts as a buffer) and inositol (an essential yeast growth factor).
The liquor (wort) is separated from the spent grain and is boiled
(with hops) to inactivate enzymes, coagulate proteins, destroy
spoilage organisms etc. The hopped wort is cooled, aerated,
and inoculated (seeded or pitched ) with a pure culture of yeast:
a strain of Saccharomyces cerevisiae (see BREWERS YEAST). A
lag period of ca. 12 h is followed by growth of the yeast. As
oxygen is used up, metabolism switches from respiratory to
fermentative, and sugars in the wort are converted to ethanol
and CO2 primarily via the EMBDENMEYERHOFPARNAS PATHWAY.
(Fermentation is exothermic, so the fermentation vessel must
be cooled.) The formation of bubbles of CO2 keeps the wort
agitated and the yeast cells in suspension. At the end of the
fermentation the yeast cells clump together see FLOCCULATION
(sense 2); in top-fermenting strains of S. cerevisiae the clumps
rise to the surface of the liquor, while those of bottomfermenting strains sediment. Most of the yeast is removed (e.g.
by surface skimming of top yeasts or collection of sediment for
bottom yeasts, and/or by centrifugation), and the beer is matured
at low temperature (e.g. 1 C); residual yeast cells (a) carry
out a secondary fermentation of remaining maltotriose, and
(b) reduce levels of diacetyl. H2 S and acetaldehyde may be
removed by purging with CO2 . Finally, the beer is filtered,
bottled or canned, and pasteurized. (See also BEER SPOILAGE.)
brick cheese See CHEESE-MAKING.
Brie cheese See CHEESE-MAKING.
bright-field microscopy See MICROSCOPY (a).
brightener See FLUORESCENT BRIGHTENER.
BrillZinsser disease See TYPHUS FEVERS.
brilliant green A yellowish-green TRIPHENYLMETHANE DYE which
contains ethyl-substituted amino groups. It has antibacterial
activity, inhibiting aerobic spore-formers more than anaerobic
spore-formers.
brilliant green agar A selective medium used for salmonellae
which have a broad host range (e.g. S. typhimurium); it contains
e.g. lactose, phenol red, and brilliant green (selective agent).
Lactose +ve colonies are green, lactose ve colonies are pink.
brinase A fibrinolysin-like PROTEASE, obtained from Aspergillus
oryzae, which can hydrolyse fibrin and fibrinogen and can lyse
blood clots. (cf. STREPTOKINASE.)
British anti-Lewisite See BAL.
brittleworts See CHAROPHYTES.
broad bean mottle virus See BROMOVIRUSES.
broad bean wilt virus A virus which may be a member of the
COMOVIRUSES but which has a wide host range and is transmitted
by aphids.
broad-range primers Primers, used in PCR, which bind to highly
conserved sequences found in the 16S rRNA gene in all bacteria;
such primers can therefore be used to detect any species of
bacterium whose 16S rRNA gene is accessible. Broad-range
primers are also referred to as universal primers.
Broad-range primers are used e.g. to study bacterial diversity
in environmental samples; the products are sequenced, and
variable regions within the amplicon (which include speciesspecific sequences) are checked against the 16S rRNA database
of known species in order to attempt identification of bacteria
within the sample.
Some PCR-based studies use broad-range primers (simultaneously with other primers) as an amplification control [see e.g.
JMM (1997) 46 773778; JCM (1999) 37 20902092].
broad-spectrum antibiotics (1) ANTIBIOTICS active against a
wide range of bacteria including both Gram-positive and
Gram-negative species. (2) Antibiotics active against a wide
range of bacteria which may include Gram-positive species,
Gram-negative species, or both.
broccoli necrotic yellows virus See RHABDOVIRIDAE.
Brochothrix
A genus of Gram-positive, facultatively anaerobic bacteria; type species: B. thermosphacta (formerly
Microbacterium thermosphactum) [IJSB (1976) 26 102104].
B. thermosphacta is common e.g. in meat and meat products (see
MEAT SPOILAGE). In young cultures cells are rod-shaped (occurring in chains), in older cultures they are small coccobacilli.
Growth conditions: 030 C (optimum ca. 2325 C); pH 59
(optimum ca. 7.0); all strains can grow in the presence of 6.5%
NaCl, many in 10% NaCl. Tests: MR +ve; VP +ve; indole
ve; H2 S ve; nitrate is not reduced, catalase +ve e.g. on
APT agar at 20 C, usually catalase ve at 30 C. During aerobic growth B. thermosphacta forms cytochromes and can use
glycerol or a range of carbohydrates as energy sources. Anaerobically, cytochromes are not formed, and glucose is fermented
primarily to L-lactic acid, acetic acid, formic acid, and ethanol
in proportions that vary with growth conditions [AEM (1983)
45 8490]. In meat under aerobic conditions B. thermosphacta
uses glucose and, when glucose is depleted, glutamate; under
anaerobic conditions only glucose can be used. (See also STAA
MEDIUM.)
[Review: Book ref. 29, pp. 139173.]
broken cream See MILK SPOILAGE.
bromatia See FUNGUS GARDENS.
bromcresol green A PH INDICATOR: pH 3.85.4 (yellow to green);
pKa 4.7.
bromcresol purple A PH INDICATOR: pH 5.26.8 (yellow to
purple); pKa 6.3.
brome mosaic virus See BROMOVIRUSES.
bromelain A basic glycoprotein thiol PROTEASE (EC 3.4.22.4)
obtained from the pineapple plant.
bromoaplysiatoxin See LYNGBYA.
5-bromo-4-chloro-3-indolyl-b-D-galactoside See XGAL.
5-bromo-4-chloro-3-indolylphosphate-p-toluidine See XP.
bromochlorophane See BISPHENOLS.
bromocresol green Syn. BROMCRESOL GREEN.
bromocresol purple Syn. BROMCRESOL PURPLE.
5-bromodeoxyuridine See BUDR.
bromophenol blue Syn. BROMPHENOL BLUE.
bromothymol blue Syn. BROMTHYMOL BLUE.
5-bromouracil (BU) A BASE ANALOGUE which, in the keto tautomeric form (which predominates), pairs with adenine (A) but
in the enol form pairs with cytosine (C). Thus, during DNA
synthesis, keto-BU may be incorporated into DNA in place of
thymine (T); if it then remains in the keto form, BU will continue to mimic T and no mutation will occur, but if it switches
to the enol form just prior to further DNA replication it will pair
with guanine (G) instead of A, leading to an AT-to-GC transition. Conversely, enol-BU may be incorporated into DNA in
place of C, and a subsequent switch to the keto form will result
in a GC-to-AT transition on subsequent DNA replication.
bromovinyldeoxyuridine (BVDU; (E)-5-(2-bromovinyl)-2 -deoxyuridine) An ANTIVIRAL AGENT which is highly active against
varicella-zoster virus; it is also active against herpes simplex
virus (HSV) type 1 (but less so against HSV type 2) and
110
Brownes tubes
with wet lesions which become dark chocolate-brown. (cf.
GINGER BLOTCH.) [Disease control by disinfection: JAB (1985)
58 259281.]
brown bodies See LEPROSY.
BrownBoveri UV-C lamp A source of high-intensity ULTRAVIOLET RADIATION; the lamp gives a radiation intensity of up to
ca. 1W/cm2 . (Conventional sources give up to ca. 10 W/cm2 .)
BrownHopps modification (of the GRAM STAIN) A procedure
used for staining bacteria in deparaffinized, hydrated tissue
sections. Essentially, sections are stained with crystal violet;
washed; treated with Grams iodine; washed; differentiated in
acetone; washed; stained with basic fuchsin; washed; treated
with Gallegos solution (an aqueous solution of formalin and
acetic acid); washed; dipped in acetone, picric acidacetone,
and acetone; and finally transferred, via xylene, to the mountant.
Gram-positive bacteria stain blue; Gram-negative bacteria stain
red. [AJCP (1973) 60 234240.]
brown oak Timber from an oak tree (Quercus sp) which has
been infected by Fistulina hepatica; such infection causes the
heartwood of the tree gradually to develop a rich brown colour.
The colour appears to derive partly from pigment within the
fungal hyphae and partly from extracellular fungal products.
Brown oak is somewhat weaker than the normal wood, but it is
valued e.g. for furniture-making.
brown rot (1) (of timber) A form of fungal TIMBER SPOILAGE
in which the CELLULOSE and HEMICELLULOSES of the wood are
decomposed while the LIGNIN remains virtually intact (although
it may be modified), leaving the wood brown, soft and friable,
and subject to cross-grain cracking. The hyphae of brown-rot
fungi (e.g. Piptoporus betulinus, Poria placenta) penetrate the
wood cell lumen and lie in contact with the inner surface
of the cell wall; a generalized thinning of the wall occurs,
suggesting a diffusion of degradative enzymes from the hyphae
(cf. WHITE ROT). A novel mechanism has been proposed for
the disruption of native cellulose by brown-rot fungi (which do
not produce exoglucanases see CELLULASES): H2 O2 , generated
by the oxidation of hexoses by glucose oxidase, is believed to
act in combination with Fe2+ (present in the wood) to oxidize
glucopyranosyl residues, causing rupture of the cellulose chains;
this could disrupt microfibrils sufficiently to allow access for
endoglucanases [Book ref. 26, pp. 2829; Book ref. 39, pp.
5659].
(2) (of fruits) A rot which affects a wide variety of
fruits particularly apples, pears and stone fruits (cherries,
plums etc) both on the tree and in storage. Soft brown lesions
develop in the fruits, initially beneath an intact epidermis; subsequently, whitish cottony pustules may develop, often in a
concentric arrangement, and the fruit eventually shrivels and
dries. Brown rots are caused by Sclerotinia spp: S. fructigena
in e.g. apples, pears and almonds, S. laxa or S. fructigena in
cherries, plums, peaches etc.
brown rust A disease of wheat and rye caused by Puccinia
recondita; orange-brown pustules, later becoming dark or black,
develop mainly on the upper (adaxial) leaf surface. On barley, a
similar disease is caused by Puccinia hordei. (See also CEREAL
DISEASES.)
Brownes tubes Sealed glass tubes containing a fluid which
changes (irreversibly) from red to green when exposed to
certain temperature/time combinations; they are used to monitor
conditions at various positions within an operating AUTOCLAVE
or hot-air oven. Type I and type II tubes are used in conventional
autoclaves and high-vacuum autoclaves, respectively; type III is
used in hot-air ovens, and type IV for monitoring exposures of
ca. 180 C/12 min. (cf. BROWNS TUBES.)
Brownian movement
biovar 2 to fuchsin. Biovars 4, 5 and 9 do not agglutinate in
A antiserum; biovars 1, 2, 3 and 6 do not agglutinate in M
antiserum. B. abortus strain 19 is similar to biovar 1 but has
reduced virulence; it is used as a live vaccine for cattle.
B. canis. Primarily a pathogen of the dog, causing e.g.
epididymitis, orchitis, prostatitis and the development of local
granulomas; man is occasionally infected. Only rough or mucoid
strains occur; these are agglutinated by R antiserum but not by
A or M antisera. Insensitive to thionin; most strains sensitive to
fuchsin. No biovars.
B. melitensis. Typically pathogenic in goats and sheep, but
also in bovines, man and pigs. Insensitive to both fuchsin and
thionin; biovar 1 is agglutinated by M antiserum, biovar 2 by A
antiserum, and biovar 3 by both A and M antisera.
B. neotomae. A non-pathogenic or weakly pathogenic species.
Acid (no gas) is formed from arabinose, galactose, glucose and
xylose. Sensitive to both fuchsin and thionin, and agglutinated
by A antiserum. No biovars.
B. ovis. A pathogen of sheep, causing epididymitis/orchitis,
or abortion in pregnant ewes. Insensitive to thionin; most strains
sensitive to fuchsin. No biovars. Smooth strains unknown;
agglutination by R antiserum only.
B. suis. Primarily a pathogen of pigs, but most or all
strains can also infect man; other hosts include e.g. dogs and
hares. Insensitive to thionin; most strains sensitive to fuchsin,
but biovar 3 is insensitive. Biovars 14 are agglutinated by
A antiserum; 4 is also agglutinated by M antiserum, and 5 is
agglutinated only by M antiserum.
An early proposal to include all strains of Brucella in a single
species (B. melitensis) [IJSB (1985) 35 292295] has not been
accepted.
Brucella ring test Syn. MILK RING TEST.
brucellin An antigenic material derived from cultures of Brucella spp.
brucellin test A SKIN TEST, analogous to the TUBERCULIN TEST,
used for detecting Brucella-induced hypersensitivity (cf. BRUCELLOSIS).
brucellosis Any human or animal disease caused by Brucella
spp. In animals the reproductive organs are generally affected,
often resulting in abortion (contagious abortion). B. abortus is
the usual causal agent in cattle, B. suis in pigs, B. melitensis
in goats, B. ovis in sheep, and B. canis in dogs, but host
specificity is not absolute. Contagious abortion in cattle (Bangs
disease) may follow infection via the mouth, vagina or wounds;
the pathogen has a predilection for the udder (resulting in its
presence in the milk) and for fetal and placental tissues (its
growth apparently being stimulated by erythritol present in these
tissues).
In man brucellosis (undulant fever, Malta fever ) is an acute
or chronic systemic disease contracted from animals via unpasteurized milk, infected carcases, etc; B. abortus, B. melitensis
or B. suis is most commonly involved. Infection occurs via the
mouth, conjunctivae or wounds. Incubation period: days, weeks
or months. Symptoms: variable, but typically include headache,
malaise, and intermittent periods of fever. Untreated cases may
persist for years. (In individuals frequently exposed to Brucella
spp disease may be due to hypersensitivity to Brucella antigens
rather than to true infection.) Lab. diagnosis: (i) Blood culture
(usually positive if blood is taken at the height of the fever).
(ii) Culture of bone marrow or lymph node aspirates (may be
useful in chronic cases). (iii) Serological assay for specific serum
agglutinins. (N.B. Agglutinins against cholera vibrios cross-react
bulgaricus milk
buccokinetal stomatogenesis See STOMATOGENESIS.
Buchnera A genus of intracellular bacteria found in the BACTERIOCYTES of aphids; aphids and Buchnera are mutually dependent neither can reproduce without the other.
The chromosome of Buchnera sp APS is one of the smallest
to be sequenced so far in bacteria (a total of 640681 base pairs)
[Nature (2000) 407 8186].
bud-fission In certain fungi (e.g. Saccharomycodes ludwigii ): a
form of BUDDING in which the septum between bud and parent
cell is almost as wide as the widest part of the parent cell.
bud scar (mycol.) See SCAR.
budding (1) (bacteriol., mycol.) In certain bacteria and fungi: a
process of cell division in which a daughter cell (or spore) develops from the mother cell as a localised outgrowth or protrusion
(bud ), the cell wall of the mature daughter cell apparently being
composed mainly of newly synthesized material; mother and
daughter cells are often physically, and sometimes functionally,
distinguishable. (cf. FISSION.) In the BUDDING BACTERIA, budding
often but not always occurs at one of the poles of the mother
cell. In some fungi (e.g. Saccharomyces cerevisiae) buds may
arise at any of a number of sites on the parent cell (multipolar
budding); in e.g. Kloeckera, buds can develop at both cell poles
(bipolar budding), while in Malassezia they can arise only at
one pole (monopolar budding). (cf. TRIGONOPSIS; see also BUDFISSION, SCAR and SPROUT MYCELIUM.)
(2) (protozool.) In some protozoa (e.g. members of the
Astomatida, Peritrichia and Suctoria): a reproductive process
in which a cell divides unequally to form a large adult and
small progeny cells (external or exogenous budding), or in which
progeny develop within the cytoplasm of the adult cell (interior
or endogenous budding).
(3) (virol.) See ENVELOPE (sense 1).
budding bacteria A diverse, non-taxonomic group of bacteria all of which undergo BUDDING; they include e.g. species
of BLASTOBACTER, CHAMAESIPHON, ENSIFER, GEMMIGER, GEODERMATOPHILUS, Hyphomicrobium, HYPHOMONAS, NITROBACTER, PASTEURIA, PLANCTOMYCES, RHODOMICROBIUM, RHODOPSEUDOMONAS
and SELIBERIA.
budgerigar fledgling disease virus A virus which causes a commercially important acute, fatal disease in fledgling budgerigars
(Melopsittacus undulatus) and may also be responsible for a
milder, chronic disease (French moult) in older birds. The virus
is apparently a POLYOMAVIRUS the first non-mammalian polyomavirus to be recorded. [Virol. (1986) 151 362370.]
BUdR (BrdU) 5-Bromo-2 -deoxyuridine: the deoxynucleoside
corresponding to 5-BROMOURACIL. It can be phosphorylated by
THYMIDINE KINASE. (cf. IDOXURIDINE.)
Buellia
A genus of crustose LICHENS (order LECANORALES).
Apothecia: lecideine, black; ascospores brown, one-septate. (cf.
DIPLOICIA; see also ENDOLITHIC.)
buffalopox virus See ORTHOPOXVIRUS.
buffy coat The thin layer of white cells which forms at the surface of the packed red cells when unclotted blood is centrifuged.
bufotenine See AMATOXINS.
bulbil (algol.) See CHAROPHYTES.
Bulbochaete
A genus of freshwater filamentous green algae
related to OEDOGONIUM. The filaments are branched and bear
long, colourless hairs, each with a bulbous base.
Bulgaria See HELOTIALES.
Bulgarian buttermilk Syn. BULGARICUS MILK.
bulgaricus milk (Bulgarian buttermilk) A beverage made by
fermenting milk with Lactobacillus bulgaricus.
with those against Brucella spp.) Chemotherapy: e.g. tetracyclines with streptomycin. (See also BRUCELLIN TEST and MILK
RING TEST.)
Bryopsis
A genus of siphonaceous green seaweeds (division
CHLOROPHYTA) which exhibit a heteromorphic alternation of
generations (cf. DERBESIA).
Bryoria
A genus of fruticose LICHENS (order LECANORALES)
separated from ALECTORIA e.g. on the basis of the smaller
colourless ascospores (8 per ascus).
BSA Bovine serum albumin.
BS-C-1 An ESTABLISHED CELL LINE derived from the kidney of an
African green monkey (Cercopithecus aethiops); the cells are
heteroploid and epithelioid.
BSE BOVINE SPONGIFORM ENCEPHALOPATHY.
BSS BALANCED SALT SOLUTION.
BssHII See RESTRICTION ENDONUCLEASE (table).
BstEII A RESTRICTION ENDONUCLEASE from Bacillus stearothermophilus; G/GTNACC.
BTB agar (bromthymol blue agar) A medium (used e.g. for
enterobacteria) containing e.g. peptone, lactose, glucose, yeast
extract, MARANIL, thiosulphate, and bromthymol blue; pH:
7.77.8. [Recipe: Book ref. 22, p. 421.]
BTEX Benzene, toluene, ethyl-benzene and xylene a group of
compounds which are sometimes present as contaminants in
aquifers. (See also BIOREMEDIATION.)
BtuB protein In Escherichia coli : an OUTER MEMBRANE protein
encoded by the btuB gene; it acts as a receptor for bacteriophage
BF23 and for various colicins, and is involved in the uptake of
VITAMIN B12 .
BtuC protein See VITAMIN B12 .
BU 5-BROMOURACIL.
bubble column fermenter A FERMENTER in which mixing and
circulation of the culture is induced by a stream of bubbles
introduced at the base of the column (which lacks a draft
tube cf. LOOP FERMENTER); it may be used e.g. with lowviscosity cultures when efficient mixing is not essential. An
increased gasliquid interface can be achieved by placing mesh
sieve plates at intervals in the column.
bubble diseases MUSHROOM DISEASES caused by Verticillium
fungicola (dry bubble) or Mycogone perniciosa (wet bubble).
[Control by PROCHLORAZ and other antifungals: PP (1983) 32
123131.]
bubble point test A test used to determine the physical integrity
of a membrane filter (see FILTRATION). In a wetted membrane,
water is retained in the pores by the forces of surface tension,
and a considerable pressure of air is needed to dislodge this
water and to force air through the pores; the minimum pressure
which can do this (the bubble point pressure) increases with
decrease in pore size, and is about 55 lb/inch2 (379 kPa) for a
membrane of pore size 0.22 m. Using the relationship between
bubble point pressure and pore size, the integrity of a membrane
of given pore size can be tested by determining its bubble point
pressure. (cf. DIFFUSION TEST.)
bubbler Syn. ALL-GLASS IMPINGER.
bubo An enlarged, inflamed lymph node (particularly in the
axilla or groin) formed e.g. in bubonic PLAGUE.
bubonic plague See PLAGUE.
buccal cavity In some ciliates: a cavity, chamber or surface
depression which is typically open to the environment and
which contains, at its base, the CYTOSTOME; the ciliature of
the buccal cavity is typically readily distinguishable from the
somatic ciliature. (See also e.g. PARORAL MEMBRANE.)
buccal overture The entrance (outer or distal region) of the
BUCCAL CAVITY.
113
bulgecin
arthropod vector (if any) etc.; the genera include BUNYAVIRUS;
HANTAVIRUS; NAIROVIRUS; PHLEBOVIRUS and UUKUVIRUS.
Bunyavirus (Bunyamwera supergroup) A genus of viruses of
the BUNYAVIRIDAE. Host range: various vertebrates; vectors: mainly
mosquitoes. MWts of L, M and S RNAs: ca. 2.73.1, 1.82.3, and
0.280.50 106 , respectively. MWts of proteins L, G1, G2 and
N: ca. 145200, 108120, 2941 and 1925 103 , respectively.
The genus comprises at least 16 serological groups, including the
Bunyamwera group (e.g. Bunyamwera virus (type species of the
genus), Cache Valley virus), the California group (e.g. CALIFORNIA
ENCEPHALITIS virus, Inkoo virus, La Crosse virus, snowshoe hare
virus), and the Simbu group (e.g. Aino virus, Akabane virus see
AKABANE VIRUS DISEASE).
bunyaviruses (1) Viruses of the BUNYAVIRIDAE. (2) Viruses of the
genus BUNYAVIRUS.
buoyant density See CENTRIFUGATION.
burdock stunt viroid See VIROID.
burdock yellows virus See CLOSTEROVIRUSES.
Burdons stain A stain for bacterial intracellular lipid. A heatfixed smear is stained with SUDAN-BLACK B for 510 min,
drained, and blotted dry. The smear is washed in xylene, blotted
dry, and counterstained for 510 sec in 0.5% aqueous safranin.
Lipid stains black, cytoplasm red. (See also NILE BLUE A.)
Burgundy mixture (plant pathol.) An agricultural antifungal
preparation which consists of a mixture of copper sulphate and
sodium carbonate; it is used in aqueous solution as a spray.
Active constituent: the COPPER ion.
Burgundy truffle See TRUFFLES.
Burkard trap See HIRST SPORE TRAP.
Burkea See MICROSPOREA.
Burkholderia
A genus of Gram-negative bacteria initially
proposed to accommodate seven (group II) species from
the genus PSEUDOMONAS, with Burkholderia (formerly Pseudomonas) cepacia as the type species [Microbiology and
Immunology (Tokyo) (1992) 36 12511275]; the other species
in this proposal were: P. mallei, P. pseudomallei, P. caryophilli,
P. gladioli, P. pickettii and P. solanacearum. Two other former
species of the genus Pseudomonas (P. plantarii and P. glumae),
and a new species, B. vandii, have since been added to the genus
[IJSB (1994) 44 235245].
(See also CYSTIC FIBROSIS.)
[B. cepacia (surface chemistry and typing methods): RMM
(1995) 6 19. B. cepacia (pathogenicity and resistance to
antibiotics): RMM (1995) 6 1016.]
Burkitts lymphoma (BL) A malignant monoclonal B-cell lymphoma which is endemic in parts of Africa where it is the
most common tumour among children. The tumours commonly develop in the mandibular and maxillary bones, but may
also develop in the ovaries, thyroid, kidneys, heart, stomach,
and spinal column. BL is associated with EPSTEINBARR VIRUS
(EBV) infection, but other factors including the occurrence of
malaria are also important in pathogenesis. BL cells contain
multiple copies of the EBV genome, and also show characteristic
chromosomal rearrangements involving reciprocal translocations
between chromosome 8 and chromosome 14 or, less frequently,
chromosome 2 or 22. These translocations apparently result in
the juxtaposition of a cellular ONCOGENE (c-myc, or possibly cmos) and the immunoglobulin (Ig) genes on chromosomes 14,
2 or 22; c-myc may be activated by the Ig gene promoter,
resulting in oncogenesis. These chromosomal rearrangements
can occur in the absence of EBV; EBV may predispose to
oncogenesis by its mitogenic effect on B cells, providing large
numbers of transformed cells and thereby increasing the chances
Butyrivibrio
of one of the three chromosomal rearrangements occurring.
Chronic malaria depresses EBV-specific cell-mediated immunity and stimulates B cell proliferation, thus potentiating the
effects of EBV. Burkitt-like lymphomas occur rarely and sporadically outside the endemic areas, and only ca. 20% of these
are associated with EBV infection.
burned spot disease (shell disease; Brandenfleckenkrankheit) A
marine CRUSTACEAN DISEASE which affects the exoskeletons of
crabs, lobsters, crayfish etc; it is caused by chitinolytic bacteria
and/or fungi which form brown erosive lesions in the calcified
chitin of the exoskeleton following damage to the epicuticle (e.g.
by abrasion). Once initiated, the lesions may support a varied
microbial flora. The disease may be fatal, but recovery may
occur if the animal survives to ecdysis. Fusarium solani has
been associated with the disease in lobsters; the fungus may
penetrate the muscles and occasionally the foregut of the lobster
[TBMS (1981) 76 2527]. (cf. BLACK GILL DISEASE.)
Burnets clonal selection theory See CLONAL SELECTION THEORY.
bursa of Fabricius In birds, a sac-like organ which develops
from the hindgut in the early embryonic stage; within the bursa,
precursors of B LYMPHOCYTES appear to undergo maturation. (See
also INFECTIOUS BURSAL DISEASE VIRUS.)
Bursaria See HETEROTRICHIDA.
bursattee Syn. EQUINE PHYCOMYCOSIS.
burst size The average number of virus particles released per
infected cell following the lytic infection of a population of
sensitive cells; it may be determined e.g. by the ONE-STEP GROWTH
EXPERIMENT (by comparing the latent period plaque count with
the plateau plaque count) or by the SINGLE BURST EXPERIMENT.
burst test A test used for assessing the strength of the seal in a
RETORT POUCH; in the test, the pouch is either inflated or is filled
with water and then compressed.
Bursulla See MYXOMYCETES.
Buruli ulcer A chronic, progressive, granulomatous skin lesion
caused by Mycobacterium ulcerans; infection occurs via wounds.
BuschkeLowenstein tumour (giant condyloma acuminatum)
A large, cauliflower-like, malignant but non-metastasizing genital tumour of humans. The genomes of HPV-6 or HPV-11 (see
PAPILLOMAVIRUS) have been identified in BuschkeL
owenstein
tumour cells [see e.g. JV (1986) 58 963966]. (cf. PAPILLOMA.)
BusseBuschke disease Syn. CRYPTOCOCCOSIS.
Bussuquara virus See FLAVIVIRIDAE.
butanediol fermentation (butylene glycol fermentation) A FERMENTATION (sense 1) carried out e.g. by certain enterobacteria, including species of Enterobacter, Erwinia, Klebsiella
and Serratia. The main products of glucose fermentation include ethanol, 2,3-butanediol and formic acid or
CO2 and H2 [Appendix III(f)]; small amounts of DIACETYL
(CH3 .CO.CO.CH3 ) may also be formed from acetolactate.
Organisms which form diacetyl or acetoin give a positive
VOGESPROSKAUER TEST. The amount of acid produced in the
butanediol fermentation is generally insufficient to give a positive methyl red test (cf. MIXED ACID FERMENTATION).
butanol fermentation Syn. ACETONEBUTANOL FERMENTATION.
butirosin An AMINOGLYCOSIDE ANTIBIOTIC.
butoconazole See AZOLE ANTIFUNGAL AGENTS.
Butschlis
granules METACHROMATIC GRANULES observed in
diatoms.
butt (microbiol.) The thickest part of a SLOPE. The butt of a
freshly-prepared slope is a microaerobic or anaerobic environment.
butt rot A TREE DISEASE in which the base (butt) of the trunk
rots. In e.g. elms (Ulmus spp) a butt rot may be caused by
116
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
C
C-type particles See TYPE C ONCOVIRUS GROUP.
C value (C-value; c ) The amount of DNA in a haploid genome;
it can be measured e.g. in picograms or in terms of the molecular
weight or the number of constituent kilobase-pairs.
C0 In the food processing industry: heating (COOKING) for 1 min
at 100 C or an equivalent amount of heat processing.
C1 cellulase See CELLULASES.
C1 compounds (1-C compounds; one-carbon compounds) Carbon compounds which contain no carboncarbon bonds and
which are more reduced than is CO2 e.g. CO, methane,
methanol, formaldehyde, formamide and formate; C1 compounds
may have more than one carbon atom: e.g. dimethyl sulphide
[(CH3 )2 S], dimethyl sulphoxide [(CH3 )2 SO], dimethyl sulphone
[(CH3 )SO2 ], trimethylamine-N-oxide [(CH3 )3 NO]. (See also
METHYLOTROPHY.)
C1 esterase inhibitor See COMPLEMENT FIXATION (a).
C1EI See COMPLEMENT FIXATION (a).
C1INH Syn. C1EI see COMPLEMENT FIXATION (a).
C2 carbon oxidation cycle See PHOTORESPIRATION.
C2a pathway See COMPLEMENT FIXATION (d).
C3 convertase See COMPLEMENT FIXATION.
C3 cycle Syn. CALVIN CYCLE.
C3bina (C3bINA) Syn. FACTOR I.
C5 convertase See COMPLEMENT FIXATION.
C27 organisms See PLESIOMONAS.
C55 lipid carrier Syn. BACTOPRENOL.
Ca2+ -ATPase See ION TRANSPORT.
Ca2+ , Mg2+ -stimulated ATPase See ATPASE.
Ca2+ transport See ION TRANSPORT.
Cabassou virus See ALPHAVIRUS.
cabbage B virus Syn. CAULIFLOWER MOSAIC VIRUS.
cabbage diseases See CRUCIFER DISEASES.
cabinet (safety cabinet) See SAFETY CABINET.
cacao diseases For diseases of the cacao plant (Theobroma
cacao) see e.g. BLACK POD DISEASE, FUSARIUM (F. decemcellulare), POD ROT, RED RUST, VASCULAR-STREAK DISEASE and WITCHES
BROOM.
cacao yellow mosaic virus See TYMOVIRUSES.
Cache Valley virus See BUNYAVIRUS.
cachectin An early name for tumour necrosis factor-a (TNF-a).
cacodylate Dimethylarsinate.
cactus virus 2 See CARLAVIRUSES.
cactus virus X See POTEXVIRUSES.
CAD See APOPTOSIS.
cAD1 See PHEROMONE.
cadang-cadang See COCONUT CADANG-CADANG VIROID.
cadaverine See e.g. DECARBOXYLASE TESTS.
cadherins A family of CELL ADHESION MOLECULES. The cadherins
are large, transmembrane glycoproteins that mediate calciumdependent homophilic cellcell adhesion (i.e. cadherin binds to
cadherin). The intracellular domain of the cadherin molecule
binds to proteins called catenins which, in turn, are linked to
the cells actin cytoskeleton.
E-cadherin occurs mainly in epithelial tissue (and in the early
stage of mammalian embryogenesis); E-cadherin is used as a
receptor for the adhesin internalin A of Listeria monocytogenes
during invasion of the intestinal epithelium. P-cadherin occurs
in the placenta and epidermis, and N-cadherin is found e.g. in
nerve and heart cells.
cadmium
calcium transport See ION TRANSPORT.
calcofluor white A FLUORESCENT BRIGHTENER which binds by
hydrogen-bonding to b-linked fibrillar polysaccharides such as
cellulose and chitin; it can be used as a fluorescent marker to
locate these polymers in cells (see MICROSCOPY (e)), and can
disrupt CELLULOSE and chitin microfibril formation in growing
cells (e.g. yeasts: [JGM (1983) 129 15771582]).
caldoactive Refers to an extreme THERMOPHILE. The term is used
more specifically by some authors to refer to an organism with
a maximum growth temperature >70 C, an optimum growth
temperature >65 C, and a minimum growth temperature >40 C
[Sci. Prog. (1975) 62 373393].
caldopentamine See POLYAMINES.
calf diphtheria See NECROBACILLOSIS.
calf pneumonia (enzootic pneumonia of calves; viral pneumonia
of calves) A non-specific calf disease, the causal agent(s) being
one or more viruses (e.g. adenoviruses, parainfluenza virus type
3, respiratory syncytial virus) frequently in association with
bacteria (e.g. Chlamydia, Mycoplasma spp); typical symptoms:
fever with constipation, followed by a mucopurulent nasal
discharge, PNEUMONIA and diarrhoea. Poor hygiene and housing
conditions (e.g. poor ventilation) and overcrowding appear to
predispose towards the disease. Mortality rates can be high e.g.
in acute RSV pneumonia.
Control involves improvements in housing etc. and chemotherapy. (See also danofloxacin in entry QUINOLONE ANTIBIOTICS.)
calf scours Scouring (see SCOURS) in young calves due to any
of a range of microbial agents, e.g. enterotoxigenic strains of
Escherichia coli, coronaviruses etc; aetiology may be complex
(e.g. mixed bacterial and viral causal agents) and the occurrence
and severity of the disease may involve both immunological and
environmental factors.
Calgitex See ALGINATE.
Caliciales A heterogeneous order of (mostly LICHEN-forming)
fungi of the ASCOMYCOTINA. Three families [Book ref. 64]:
Caliciaceae. Mostly lichen-forming (photobiont: a green alga).
Thallus thin crustose or immersed in the substratum (usually
wood or bark). Apothecia (mazaedia) stalked or sessile. Lichenforming genera include e.g. Calicium, Chaenotheca, Coniocybe,
Cyphelium.
Mycocaliciaceae. Lichenicolous or fungicolous (possibly also
lichen-forming) fungi in which the thallus is immersed in
the substratum or absent. Apothecia stalked, asci thick-walled
(mazaedia are not formed). Genera: e.g. Stenocybe.
Sphaerophoraceae. All lichen-forming (photobiont: a green
alga). Thallus foliose or fruticose. Apothecia (mazaedia) often
globose, marginal or terminal. Genera: e.g. Sphaerophorus.
Calicium See CALICIALES.
Caliciviridae A family of VIRUSES which infect vertebrates; caliciviruses were formerly classified as a genus in the family
Picornaviridae. The virions are non-enveloped, roughly spherical, ca. 3539 nm diam., and have 32 characteristic cupshaped surface indentations arranged with icosahedral symmetry observable by electron microscopy of negatively stained
preparations. The capsid contains a single major polypeptide
species (MWt ca. 6000071000) and a minor polypeptide (MWt
ca. 15000). Genome: one molecule of positive-sense ssRNA
(MWt ca. 2.62.8 106 ) which is apparently polyadenylated
at the 3 end but not capped at the 5 end; the RNA is covalently linked (possibly at its 5 end) to a protein (MWt ca.
1000015000) which is necessary for infectivity. Replication
occurs in the cytoplasm; dsRNAs (presumably replicative intermediates), genome-sized ssRNAs, and subgenomic ssRNAs can
CAMP test
bacterial growth (apparently by withholding zinc ions), and
this may antagonize certain antibiotics (e.g. b-lactams) used for
chemotherapy. [Zinc in antimicrobial defence: RMM (1997) 8
217224.]
Calvatia See LYCOPERDALES.
Calvin cycle (CalvinBenson cycle, or BensonCalvinBassham
cycle; reductive pentose phosphate cycle; C3 cycle) A cyclic
pathway used for the fixation of CARBON DIOXIDE by a wide
range of AUTOTROPHS (q.v.). (See also METHYLOTROPHY.) The
key enzymes in the Calvin cycle are RIBULOSE 1,5-BISPHOSPHATE
CARBOXYLASEOXYGENASE (RuBisCO), responsible for the CO2 fixing reaction, and phosphoribulokinase (ribulose 5-phosphate
kinase, EC 2.7.1.19), responsible for regenerating the CO2
acceptor: ribulose 1,5-bisphosphate (RuBP). For every three
molecules of CO2 fixed, six molecules of 3-phosphoglycerate are
formed; of these, five are required for the regeneration of RuBP,
while the remaining molecule is available as a source of carbon
for biosynthesis (see figure on page 120). The ATP and reduced
NAD(P) required to drive the cycle are supplied by the light
reactions of PHOTOSYNTHESIS in phototrophs, or by the oxidation
of reduced inorganic compounds in CHEMOLITHOAUTOTROPHS.
[Regulation of the Calvin cycle in bacteria: AvL (1984) 50
473487.] (See also PHOTORESPIRATION.)
calyciform Cup-shaped.
calymma See RADIOLARIA.
Calymmatobacterium
A genus (incertae sedis) of Gramnegative bacteria which occur as pathogens in man (see GRANULOMA INGUINALE). Cells: non-motile, pleomorphic, capsulated,
round-ended rods, 0.51.5 1.02.0 m. In exudates from diseased tissues the cells are usually seen in the cytoplasm of large
mononuclear phagocytes. The organisms can be cultured in the
chick embryo yolk sac or on specialized egg yolk-containing
media. Optimum growth temperature: 37 C. Type (only) species:
C. granulomatis. [Book ref. 22, pp. 585587.]
Calyptralegnia See SAPROLEGNIALES.
CAM (1) Chorioallantoic membrane: see EMBRYONATED EGG.
(2) CELL ADHESION MOLECULE.
cam gene See METHANOGENESIS.
CAM plasmid An IncP-2 Pseudomonas PLASMID (ca. 500 kb)
which encodes the capacity for metabolization of camphor
(compare TOL PLASMID).
cAM373 See PHEROMONE.
camalexin A PHYTOALEXIN (a substituted indole) produced by
Arabidopsis.
Camarops See SPHAERIALES.
Camarosporium A genus of fungi of the class COELOMYCETES.
(See also LEPTOSPHAERIA.)
camelpox virus See ORTHOPOXVIRUS.
Camembert cheese See CHEESE-MAKING.
cAMP CYCLIC AMP.
cAMPCAP See CATABOLITE REPRESSION.
CAMP factor See CAMP TEST.
cAMP phosphodiesterase See ADENYLATE CYCLASE.
cAMP receptor protein See CATABOLITE REPRESSION.
CAMP test (ChristieAtkinsMunch-Petersen test) A test used
for the presumptive identification of group B streptococci. (Some
group A streptococci may also give a positive test, particularly
under anaerobic conditions [Book ref. 46, pp. 15901591].) The
organism under test is inoculated in a fine streak on the surface of
ox- or sheep-blood agar; a second streak perpendicular to the
first but separated from it by a few millimetres is made with
a culture of a b-HAEMOLYSIN-producing strain of Staphylococcus
aureus. The plate is then incubated (aerobically) for ca. 12 hours
Campanella
6NAD (P)H + 6H
6ATP
COOH
3[CO2 ]
CH2O
6NAD (P)
COO P
3-phosphoglycerate
kinase
CH2O
3-phosphoglycerate
6Pi BIOSYNTHESIS
HCOH
triose phos
p h at
ed
1,3-bisphosphoglycerate
ehy
dr
og
Co
Bis
Ru
HCOH
6ADP
en
as
CH2O P
3
t
ke
ns
tra
HCOH
HCOH
CO
1
CHO
CH2O
sedoheptulose
7-phosphate
CH2OH
ribose phosphate
isomerase
HOCH
fructose
1,6-bisphosphatase
H2O
sedoheptulose
HCOH
CO
HCOH
HOCH
1,7-bisphosphate
aldolase
CH2O P
ribulose
5-phosphate
CHO
HCOH
HCOH
1
H 2O
sedoheptulose
1,7-bisphosphate
erythrose
4-phosphate
CH2OH
CO
1
CH2OH
HOCH
HCOH
HCOH
CO
2
fructose
1,6-bisphosphatase
Pi
HCOH
CH2O P
CH2O P
phosphoketopentose
epimerase
CH2O P
fructose
1,6-bisphosphate
HCOH
HCOH
HCOH
HCOH
CH2O P
CO
3
CH2O P
CO
Pi
ribose
5-phosphate
CH2O P
fructose
1,6-bisphosphate
aldolase
CH2O P
HCOH
HCOH
dihydroxyacetone
phosphate
HCOH
HCOH
glyceraldehyde
3-phosphate
CO
CH2O
HCOH
HCOH
3ADP
HCOH
trios
om
te is
ha
osp
e ph
CH2OH
HOCH
ribulose
1,5-bisphosphate
3ATP
CHO
eras
CH2OH
CH2O P
phosphoribulokinase
as
ol
CO
CH2O P
HOCH
HCOH
tra n
CH2O P
fructose
6-phosphate
sketola s e
xylulose 5-phosphate
CALVIN CYCLE. For simplicity, the intermediate withdrawn for biosynthesis is shown as glyceraldehyde 3-phosphate. In reality, other
intermediates may be withdrawn. For example, 3-phosphoglycerate is a precursor for the synthesis of various amino acids, fatty acids, purines
and pyrimidines; withdrawal of 3-phosphoglycerate rather than glyceraldehyde 3-phosphate reduces the immediate energy cost of the cycle
by 1 ATP and 1 NAD(P)H per 3 CO2 fixed.
Candida
in humans with gingivitis, periodontitis etc., but apparently nonpathogenic.
C. fetus. Cells appear comma- or S-shaped or gull-winged.
(Loosely wound spiral filaments (up to 8 m in length) occur
in old cultures.) Catalase +ve. Hydrogen sulphide (TSI) ve.
Growth occurs at 25 C but not at 42 C. Hippurate and indoxyl
acetate are not hydrolysed. Pathogenic.
C. jejuni. Cells: small, tightly coiled spirals. On exposure of
cultures to air, coccoid bodies form rapidly. SWARMING occurs
on moist agar (the DIENES PHENOMENON does not occur). Catalase
+ve. Hydrogen sulphide (TSI) ve. Growth occurs at 42 C but
not at 25 C. Hippurate and INDOXYL ACETATE are hydrolysed.
Pathogenic. [PCR-RFLP typing of C. jejuni : LAM (1996) 23
163166; PGFE typing of Penner HS11 strains of C. jejuni :
JMM (1998) 47 353357.]
C. pylori. Re-classified: see HELICOBACTER.
C. sputorum. Cells: slender, curved rods, appearing commashaped, gull-winged or occasionally filamentous. Catalase ve.
Hydrogen sulphide (TSI) +ve. Growth occurs at 42 C (except
for subsp bubulus) but not at 25 C (except for some strains
of subsp bubulus). Hippurate and indoxyl acetate are not hydrolysed. Subsp bubulus and sputorum can grow anaerobically with
fumarate; subsp mucosalis requires hydrogen or formate (as well
as fumarate) for anaerobic growth. Subsp bubulus occurs in the
genital tract in cattle and sheep, apparently as a commensal.
Subsp mucosalis is found in pigs, apparently as a commensal in
the mouth and as a pathogen, causing enteric disease. Subsp
sputorum occurs in the gingival crevice flora of man but is
apparently non-pathogenic.
(See also ARCOBACTER and HELICOBACTER.)
[Book ref. 22, pp 111118. Culture, media etc.: Book
ref. 219, pp 444446. Campylobacter spp (genotyping: minireview): AEM (2000) 66 19.]
Campylobacteraceae A family comprising the genera ARCOBACTER and CAMPYLOBACTER.
campylobacteriosis (med., vet.) Any human or animal disease
caused by a strain of CAMPYLOBACTER.
In man, disease is commonly food-borne, and is usually
caused by C. jejuni or C. coli ; less frequently isolated pathogens
include C. hyointestinalis and C. upsaliensis. Typically, disease
involves diarrhoea/enterocolitis, but disseminated infection can
occur in the immunocompromised patient, and meningitis may
develop in neonates. The usual sources of infection are inadequately cooked meats, especially poultry, unpasteurized milk
and untreated (or contaminated) water; cross-contamination of
food, particularly from raw (uncooked) poultry, is an important
factor. The incubation period (17 days) may be followed by
several days of watery diarrhoea, often with abdominal pain.
In severe cases the diarrhoea may be bloody; in some cases,
symptoms resemble those of acute ulcerative colitis. In a small
number of cases patients subsequently develop reactive arthritis;
very rarely they develop the GUILLAINBARRE SYNDROME.
Chemotherapy. For persistent cases: erythromycin or e.g.
ciprofloxacin.
[Campylobacter infections (reviews): RMM (1997) 8 113
124; Microbiology (1997) 143 521.]
In animals, campylobacters are commonly found as commensals in the gut. However, C. fetus can cause abortion in sheep
(and less often in cattle). The venerealis subspecies of C. fetus
causes abortion and infertility in cattle, while C. sputorum subsp
mucosalis causes enteric disease in pigs. (See also WINTER DYSENTERY.)
CaMV CAULIFLOWER MOSAIC VIRUS.
candidate virus
of whitish mucoid plaques on the mucous membranes. (See
also NON-GONOCOCCAL URETHRITIS.) Cutaneous candidiasis tends
to occur on skin areas constantly exposed to moisture, regions
commonly affected including e.g. the groin and axillae (see also
PARONYCHIA); infected skin is swollen, red and pruritic. Chronic
mucocutaneous candidiasis is a severe condition which occurs
in immunocompromised or otherwise abnormal individuals;
the skin and mucous membranes of the entire body may be
affected, with chronic, granulomatous, inflammatory reactions
in the underlying tissues. Other forms of candidiasis include
bronchocandidiasis, pulmonary candidiasis (often secondary
to other diseases), and systemic candidiasis (involving e.g.
fungaemia, endocarditis, nephritis etc cf. TORULOPSOSIS). Lab.
diagnosis: microscopical and cultural examination of material
from lesions etc (see CANDIDA).
In animals, candidiasis may involve the intestinal tract, skin,
and/or various internal organs (see also MASTITIS); in calves
and piglets the intestine is usually involved, and infection
can cause watery diarrhoea, anorexia, dehydration, and even
death. In birds, candidiasis commonly involves the digestive
tract particularly the crop.
[Book ref. 103.]
candidosis Syn. CANDIDIASIS.
candle (verb) To carry out CANDLING.
candle filter See FILTRATION.
candle jar A container within which cultures etc can be incubated under an increased partial pressure of CO2 ; the CO2 is
provided by placing a lighted candle in the container prior to
closure.
candle-snuff fungus See XYLARIA.
candling (virol.) A procedure for observing the contents of an
intact egg by transmitted light. An EMBRYONATED EGG is placed
over an aperture in a box containing an electric lamp; internal
details of the egg such as the positions of the embryo and
blood vessels can be seen, thus facilitating the inoculation of
a particular membrane or cavity of the egg. Candling is best
performed in a darkened room, and should be carried out rapidly
to avoid overheating the egg.
cane blight In raspberry canes: a disease caused by Leptosphaeria coniothyrium. Infection occurs mainly via wounds;
leaves shrivel and die, dark patches appear on the stem bases,
and bark associated with these patches cracks open.
cane-cutters disease LEPTOSPIROSIS caused by L. interrogans
serotype australis A; the disease is common among cane-cutters
in N. Queensland, Australia.
cane gall A disease of Rubus spp (raspberry, blackberry etc) in
which small spherical galls or elongated ridges develop on the
stems. Causal agent: Agrobacterium rubi.
cane spot (of raspberry) See ELSINOE .
canicola fever LEPTOSPIROSIS caused by L. interrogans serotype
canicola.
canid herpesvirus 1 See ALPHAHERPESVIRINAE.
canine distemper An acute, infectious disease of dogs and
other animals (e.g. foxes, mink, raccoons, wolves) caused by
a virus of the genus MORBILLIVIRUS. Infection occurs mainly
by droplet inhalation, also e.g. by ingestion. Incubation period:
ca. 330 days. Symptoms initially include fever, nasal and
ocular discharge, and listlessness. The fever subsides, then recurs
with vomiting, diarrhoea, and often pneumonia; signs of CNS
involvement (e.g. fits) may occur. (cf. HARD-PAD.) The disease
affects mainly young animals. However, persistent infection
may result in old dog encephalitis a condition characterized
by progressive neurological degeneration. The distemper virus
Cantharellales
has also been associated (rarely) with a demyelinating disease
in man.
Effective anti-distemper vaccines are available.
canine herpesvirus See ALPHAHERPESVIRINAE.
canine parvovirus A subspecies of the feline parvovirus (genus
PARVOVIRUS) which appeared initially in Europe and then spread
rapidly in 1978, causing worldwide outbreaks of disease in dogs.
Infection may occur via the nasopharynx or via lymphoid tissues,
including the tonsils. Viraemia leads to generalized infection of
lymphoid tissues. Levels of erythrocytes (red blood cells) are not
affected, and panleukopenia is infrequent in the dog (cf. FELINE
PANLEUKOPENIA VIRUS). Infection of dividing epithelial cells in
the ileum and jejunum impairs osmotic regulation and leads
to diarrhoea (often containing blood/mucus); large numbers of
virions are shed during the diarrhoeal phase. The disease can be
associated with high mortality rates, but the severity varies in
individual animals some infections being mild/subclinical.
In neonatal puppies there is no manifestation of enteritis. In
these animals infection may lead to death from myocarditis,
often at 38 weeks of age (but sometimes up to 4 months of
age). Onset of disease is rapid, typically with cardiac arrhythmia,
pulmonary oedema and dyspnoea; the myocardium suffers multifocal necrosis. Infrequently, infection of the neonatal animal
gives rise to lesions in a variety of tissues.
Canine parvovirus is apparently distinct from the minute virus
of canines (sometimes also called canine parvovirus) a virus
which is widespread in canine populations and which can be
isolated from the faeces of asymptomatic dogs.
[Pathogenesis of canine parvovirus: BCH (1995) 8 5771.]
canker (plant pathol.) An imprecise term usually used for a plant
disease which is characterized (in woody plants) by the death of
cambium tissue and resulting loss and/or malformation of bark,
or (in non-woody plants) by the formation of sharply delineated,
dry, necrotic, localized lesions on the stem. (The term canker
may also be used to refer to the lesion itself, particularly in
woody plants.) Cankers may be caused by bacteria (e.g. bacterial
canker of cherry and plum is caused by Pseudomonas syringae
pv. morsprunorum) or fungi (see e.g. APPLE CANKER, BEECH BARK
DISEASE, BLEEDING CANKER, PITCH CANKER).
canning A form of APPERTIZATION in which, typically, suitably
prepared foods are put into metal containers (cans, tins)
which are then exhausted, hermetically sealed, and heated; as
an alternative, the food may be heat-treated before being placed
aseptically in pre-sterilized cans which are then sealed under
aseptic conditions. Most cans are made of tinplate (tin-plated
steel) see also TIN but aluminium or other materials (e.g.
lacquered tin-free steel) may be used. (See also RETORT POUCH.)
(a) The canning process. Conventional canning involves the
following stages.
Food preparation. According to the type of food, this may
involve grading, cutting, peeling, blanching (see also INDIVIDUAL
QUICK BLANCH), washing etc; foods for canning must be as free
as possible from microbial contamination because the efficacy
of heat treatment is related to the level of contamination.
Filling the cans. This process must take into account the
fact that the efficiency of subsequent processes depends on the
correct volume of free space (headspace) between the surface
of the food and the top of the can.
Exhausting the cans. The removal of air reduces the strain on
the can during subsequent heating and inhibits long-term internal
corrosion. Exhausting may be carried out by heating immediately
prior to sealing, by sealing cold food into the can under vacuum
(vacuumizing), or by injecting steam into the headspace during
the sealing process.
Cantharellus
by a motile cell on contact with a surface. In Dictyostelium
discoideum, capping appears to involve interaction between
ACTIN microfilaments (which are linked, through the cytoplasmic
membrane, to patches of ligand) and cortical MYOSIN [JCB
(1985) 100 18841893]. (See also DYSENTERY (b).)
caprine arthritisencephalitis (CAE) A disease of goats caused
by a retrovirus of the LENTIVIRINAE; symptoms include interstitial
pneumonia, leucoencephalitis, inflammatory lesions in the CNS,
and a progressive arthritis.
caprinized vaccine A VACCINE containing live organisms whose
virulence for a given host species has been attenuated by SERIAL
PASSAGE through goats.
Capripoxvirus (sheep-pox subgroup) A genus of viruses of the
CHORDOPOXVIRINAE which cause disease in ungulates (see e.g.
GOAT POX, LUMPY SKIN DISEASE and SHEEP POX); capripoxviruses
can be transmitted mechanically by arthropod vectors. The
virions are longer and narrower than those of orthopoxviruses;
haemagglutinin is not produced, and infectivity can be destroyed
e.g. by ether. The viruses in this group are very closely related
serologically [JGV (1986) 67 139148].
capsduction A mode of gene transfer in strains of Rhodopseudomonas capsulata: DNA transfer from donor to recipient is
mediated by a phage-like particle known as the gene transfer agent (GTA). Although the GTA morphologically resembles a tailed bacteriophage (head: apparently icosahedral, ca.
30 nm diam., with short spikes; tail: variable in length, bearing tail fibres) no phage-specific DNA has been detected;
the linear dsDNA (MWt ca. 3 106 ) carried by the GTA is
derived entirely from the host cell (chromosome or plasmid),
and any region of the host genome can be packaged. Strains
of R. capsulata which do not naturally produce GTA can act as
recipients in capsduction but do not acquire the ability to produce
GTA in consequence. Capsduction has been useful for mapping
and genetic analysis in R. capsulata. (cf. TRANSDUCTION.)
capsid In a virion: a protein coat or shell which surrounds either
the nucleic acid genome or a nucleoprotein CORE; it commonly
exhibits ICOSAHEDRAL SYMMETRY. (See e.g. ADENOVIRIDAE.) In
some viruses the capsid is itself surrounded by an ENVELOPE
(see e.g. TOGAVIRIDAE). (cf. NUCLEOCAPSID.)
capsidiol A PHYTOALEXIN (a derivative of 5-epiaristolochene)
produced e.g. by the tobacco and green pepper plants.
capsomer (capsomere) See ICOSAHEDRAL SYMMETRY.
capsule (1)(a) In prokaryotes, a layer of material external to
but contiguous with the CELL WALL; the term thus includes
any polysaccharide and/or protein surface layer(s) (including
the bacterial S LAYER) but excludes those S layers which
constitute the cell wall proper in members of the Archaea. (cf.
GLYCOCALYX.) In some bacteria (e.g. Beijerinckia) a capsule may
enclose more than one cell.
Capsules are commonly divided into three categories.
(i) Macrocapsules or true capsules are sufficiently thick to
be easily visible (with negative staining see CAPSULE STAIN)
on light microscopy. (ii) Microcapsules cannot be observed by
light microscopy, but their presence may be revealed by electron
microscopy or by serological techniques (see e.g. QUELLUNG
PHENOMENON); some bacteria which have lost the ability to form
a macrocapsule may form a serologically identical microcapsule.
(iii) Slime layers are diffuse secretions which may adhere
loosely to the cell surface; slime layers commonly diffuse into
the medium when the organism is grown in liquid culture, and
may be too permeable to stains to be observable by microscopy.
(Since capsules normally contain a high proportion of water,
they may not be detectable in specimens dehydrated prior to
microscopy.)
e.g. in Cantharellus infundibuliformis and Craterellus cornucopioides) or stalked and pileate; the hymenophore may be
smooth, wrinkled, or lamella-like. Cantharellus cibarius (the
chanterelle) is an edible species which forms a deep yellow,
flat or centrally concave pileus on a stipe which tapers towards
the base; the gills are yellow, forked and decurrent, and the
basidiospores are ochre, ellipsoidal, ca. 810 5 m.
Cantharellus see CANTHARELLALES.
cap (1) (mycol.) The PILEUS of a mushroom-shaped fruiting body.
(2) (mol. biol.) See MRNA (b). (3) See CAPPING sense 3.
CAP Catabolite activator protein: see CATABOLITE REPRESSION.
cap-binding protein See MRNA (b).
capacity test A type of test used to determine the capacity of
a DISINFECTANT to retain activity in the presence of increasing
numbers of bacteria. Essentially, aliquots of a bacterial suspension are periodically added to a fixed volume of disinfectant
solution which is subcultured (to detect viable bacteria) at fixed
intervals of time after the addition of each aliquot. (See e.g.
KELSEYSYKES TEST.)
capillitium A system of (non-cellular) threads or filaments which
ramify through the spore mass in the fruiting bodies of certain slime moulds of the MYXOMYCETES and fungi of the GASTEROMYCETES. In myxomycetes, the capillitial threads may be
solid or hollow, free or interconnected, smooth or ornamented,
and in certain species they may bear nodes or encrustations of
lime (see e.g. FULIGO); the nature of the capillitium is an important taxonomic feature. At least some types of capillitium may
aid in spore dispersal; some are elastic, helping to expose spores
when the peridium ruptures, while others are hygroscopic, their
movements in response to changes in humidity helping to dislodge and release the spores.
capneic Syn. CAPNOPHILIC.
Capnocytophaga A genus of Gram-negative, capnophilic GLIDING BACTERIA found in the human oral cavity and associated with
e.g. PERIODONTITIS, abnormalities in neutrophil function, and in
compromised patients systemic disease. The organisms are
flexible fusiform rods, ca. 0.30.5 38 m. Metabolism: fermentative (glucose being fermented to succinic and acetic acids)
or respiratory (with O2 as terminal electron acceptor). Although
CO2 may be required for initial isolation, high levels of CO2
are not necessarily required for fermentation or oxidation of glucose [IJSB (1985) 35 369370]. Agar is not liquefied. Optimum
growth temperature: 37 C. Species: C. gingivalis, C. ochracea
(formerly Bacteroides ochraceus), and C. sputigena.
Capnodium See SOOTY MOULDS.
capnophilic Refers to any organism whose growth either
requires, or is stimulated by, higher-than-atmospheric levels of
carbon dioxide.
capped mRNA See MRNA (b).
capping (1) See MRNA (eukaryotic).
(2) The binding of a specific protein or agent to the
end of an ACTIN microfilament or a microtubule (see MICROTUBULES), resulting e.g. in cessation of polymerization/assembly
at that end.
(3) In some types of eukaryotic cell: a process which
is initiated when cell-surface molecules are cross-linked by
multivalent ligands (e.g. antibodies, lectins). The cross-linked
molecules from different regions of the cell surface initially
cluster into groups or patches (patching); subsequently, all the
patches undergo an ATP-dependent translocation to one pole of
the cell, forming a cap (capping). Capping appears to occur
only in cells capable of motility, and it has been suggested
that it is the expression of a response similar to that given
124
carbomycin
capsule stain Bacterial CAPSULES may be demonstrated e.g. by
negative STAINING: bacterial growth is mixed with a loopful of
e.g. India ink or aqueous NIGROSIN on a clean slide and overlaid
with a cover-glass; under the high-dry or oil-immersion objective
the capsule appears as a clear zone between the cell wall and
the dark background.
capsule swelling reaction Syn. QUELLUNG PHENOMENON.
captafol (difolatan; N-(1,1,2,2-tetrachloroethylthio)-cyclohex-4ene-1,2-dicarboximide) An agricultural antifungal agent related
to CAPTAN; it is used as a PROTECTANT e.g. against late blight of
potato.
captan An antibacterial and ANTIFUNGAL AGENT (N-(trichloromethylthio)-cyclohex-4-ene-1,2-dicarboximide) widely used as
an agricultural PROTECTANT; it is effective against a number
of fungal plant pathogens, and is used e.g. for the prevention
of apple scab and leaf-spot diseases (such as black spot of
roses), and as a component of seed dressings. The activity of
captan has been attributed to the SCCl3 group which may
react with essential SH groups within the fungal cell. Captan is
almost insoluble in water and is often formulated as a WETTABLE
POWDER. (cf. CAPTAFOL.)
carate Syn. PINTA.
carbamate kinase See e.g. ARGININE DIHYDROLASE.
carbamic acid derivatives (as antimicrobial agents) Antimicrobial derivatives of carbamic acid (NH2 COOH) include UREA,
derivatives of thiocarbamic acid, NH2 .CS.OH (e.g. TOLNAFTATE),
and DITHIOCARBAMATES. (See also BENOMYL.)
carbamide Syn. UREA.
carbanilides (as antimicrobial agents) Carbanilide (diphenyl
urea, (C6 H5 NH)2 CO) and substituted carbanilides (e.g. 3,4,4 trichlorocarbanilide, TCC, = triclocarban) are active mainly
against Gram-positive bacteria; they appear to affect the
functioning of the cytoplasmic membrane. TCC is also active
against certain fungi (e.g. Trichophyton spp).
carbapenems A class of b-LACTAM ANTIBIOTICS (q.v. for structure) produced (extracellularly) by Streptomyces spp; in addition to possessing antibacterial activity, many carbapenems are
inhibitory to b-LACTAMASES. (cf. CLAVULANIC ACID.) Carbapenems are stable in aqueous solution near neutral pH. They
include e.g. asparenomycins, epithienamycins, olivanic acids,
pluracidomycins, PS-5, and THIENAMYCIN.
carbendazim (MBC) An agricultural antifungal agent the
active derivative of many of the BENZIMIDAZOLES. Carbendazim
is used e.g. in the treatment of eyespot of wheat and barley
and (as a seed treatment) as a protectant against damping off
caused by Rhizoctonia solani. It is often mixed with other antifungal agents e.g. PROPICONAZOLE or PROCHLORAZ for use as
a broad-spectrum antifungal preparation.
carbenicillin See PENICILLINS.
carbofuran A broad-spectrum carbamate insecticide used as a
soil treatment for the control of insect pests on a range of crop
plants. The persistence of carbofuran in the field is limited owing
to the wide range of soil microorganisms which can degrade the
compound [FEMS Ecol. (2000) 34 173180].
carbolfuchsin A red dye used e.g. in the GRAM STAIN and in
ZIEHLNEELSENS STAIN. Concentrated carbolfuchsin is made by
adding 10% basic FUCHSIN in 95% ethanol (10 ml) to 5%
aqueous phenol (100 ml); the solution is filtered after standing
overnight.
carbolic acid Syn. phenol (see PHENOLS).
carbolic soap See SOAPS.
Carbomyces See PEZIZALES.
carbomycin See MACROLIDE ANTIBIOTICS.
carbon cycle
an imbalance in carbon cycling may mean that periods of net
autotrophy (when autotrophic fixation of carbon dioxide exceeds
bacterial respiratory output) may occur at different times of
the year to compensate for periods of net heterotrophy [Nature
(1997) 385 148151].
Carbon cycling is relevant to the GREENHOUSE EFFECT. Moreover, the evolution of the carbon cycle is an interesting topic in
itself [FEMS Reviews (1992) 103 347354].
carbon dioxide (CO2 ) (a) CO2 as a food preservative. CO2
(550%) inhibits the growth of many types of microorganism and is used in FOOD PRESERVATION e.g. for meats (see
MEAT SPOILAGE), fish, fruit and vegetables (in which CO2 also
extends storage life e.g. by delaying ripening), and for carbonated beverages. In general, CO2 inhibits moulds more than
yeasts, Gram-negative bacteria more than Gram-positive species.
CO2 dissolves in water to form carbonic acid, H2 CO3 , which
dissociates to form H+ and HCO3 (pK 6.37); some inhibition
may thus be due to a pH effect. However, CO2 also exerts a
direct antimicrobial effect which is largely independent of either
pH or oxygen concentration. The mechanism of this effect is
unknown, but direct inhibitory effects of CO2 on certain enzymes
have been reported; it has also been suggested that CO2 dissolves
tio n
CO2
photo
auto
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animals
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CARBON CYCLE: simplified scheme showing some of the major interconversions of carbon in nature (see entry). Bacteria have significant
roles, as both autotrophs and heterotrophs, and certain members of the Archaea have unique roles as methanogens; the methylotrophs
include methane-utilizing bacteria. Various microorganisms, including bacteria and fungi, are responsible for the essential conversion of dead
organic carbon to biomass and carbon dioxide; without this process the cycle would stop.
Reproduced from Bacteria 5th edition, Figure 10.1, page 256, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
126
carcinogen
aspects: MS (1986) 3 149153. Biochemistry and physiology:
FEMS Reviews (1986) 39 161179.]
The oxidation of carbon monoxide to carbon dioxide is catalysed by an enzyme sometimes referred to as CO dehydrogenase
(a CO OXIDASE); the cytochrome oxidase of one branch of the
respiratory chain is insensitive to inhibition by carbon monoxide. The carbon dioxide produced is assimilated via the CALVIN
CYCLE. In at least some cases it appears that the CO oxidase
is functional only when attached to a membrane-bound electron
acceptor (cytochrome b561 ) the ability of the cells to oxidize
carbon monoxide being lower during the stationary phase when
some of the enzyme is cytoplasmic [FEMS Reviews (1993) 104
332336].
Many or all of the carboxydobacteria are able to obtain energy
by the oxidation of hydrogen, and can grow more rapidly with
hydrogen/carbon monoxide/oxygen mixtures than with mixtures
of carbon monoxide and oxygen.
At least some species are facultatively heterotrophic.
The organisms occur e.g. in soil and polluted waters, sewage
etc. Species include e.g. Bacillus schlegelii, Pseudomonas carboxydohydrogena, P. carboxydovorans and P. thermocarboxydovorans.
The carboxydobacteria were once classified as methylotrophs
(users of C1 compounds) but are now excluded from this
category as they do not produce/assimilate formaldehyde.
carboxymethylcellulose See CM-CELLULOSE.
carboxypeptidase See PROTEASES.
carboxysomes Intracellular polyhedral bodies (typically ca.
90500 nm diam.) found in many autotrophic prokaryotes:
e.g., in Thiobacillus intermedius, T. neapolitanus, T. thiooxidans
and T. thioparus (but not in T. novellus or T. versutus); in
Nitrobacter winogradskyi and a marine species of Nitrosomonas (but not in Nitrospina gracilis or Nitrosococus
mobilis); apparently in Rhodomicrobium vannielii (but not
in green bacteria or purple non-sulphur bacteria); in most
or all cyanobacteria (in vegetative cells and akinetes but
not in heterocysts); in Prochloron; and apparently in many
cyanelles. Carboxysomes from T. neapolitanus each consist
of a number of doughnut-shaped particles (ca. 10 nm diam.)
enclosed within a single-layered membrane or shell; these particles are molecules of RIBULOSE 1,5-BISPHOSPHATE CARBOXYLASEOXYGENASE (RuBisCO). Carboxysomes from other organisms appear to resemble those of T. neapolitanus, and RuBisCO
has been found in all carboxysomes in which it has been
sought (e.g. in those from Anabaena cylindrica, Chlorogloeopsis fritschii, Nitrobacter sp, Nitrosomonas sp). The function of
carboxysomes is unknown. [Biol. Rev. (1984) 59 389422.]
carbuncle A cluster of interconnected BOILS in which PUS is
eventually discharged via several openings. It is usually caused
by Staphylococcus aureus.
Carchesium A genus of sedentary ciliate protozoa (subclass PERITRICHIA). Carchesium occurs in various freshwater and marine
habitats, and some species (e.g. C. polypinum) are common
in SEWAGE TREATMENT plants. (See also SAPROBITY SYSTEM and
SEWAGE FUNGUS.) In size and shape Carchesium resembles VORTICELLA e.g. it has a bell-shaped zooid: however, Carchesium is
a colonial peritrich the mature organism consisting of a number of zooids carried on a branching stalk, each zooid and its
individual branch of the stalk being capable of independent contraction.
carcinogen (1) Any agent which can cause CANCER. In general,
carcinogens appear to exert their effect by interacting with the
DNA of the target cell; many carcinogens are also mutagens.
carcinoma
carnation latent virus See CARLAVIRUSES.
carnation mottle virus See TOMBUSVIRUSES.
carnation necrotic fleck virus See CLOSTEROVIRUSES.
carnation ringspot virus See DIANTHOVIRUSES.
carnation vein mottle virus See POTYVIRUSES.
carnidazole See NITROIMIDAZOLES.
carnivorous Refers to protozoa which feed on other protozoa,
crustacea, etc. (cf. HERBIVOROUS.)
Carnobacterium A genus of heterofermentative LACTIC ACID BACTERIA found e.g. on vacuum-stored chilled meats and on meats
stored in a carbon-dioxide-rich environment. Carnobacterium
spp have been studied e.g. as sources of BACTERIOCINS. [Bacteriocin production by C. piscicola: JBC (1994) 269 1220412211.
Divercin V41, a new bacteriocin from C. divergens V41: Microbiology (1998) 144 28372844.]
Carnoys fluid A FIXATIVE: either (a) ethanol (95% or 100%) and
glacial acetic acid in the ratio 3:1, or (b) ethanol (95% or 100%),
chloroform, and glacial acetic acid (6:3:1).
carotenes See CAROTENOIDS.
carotenoid band shift A light-induced change in the absorption
spectrum of a photosynthetic membrane due, mainly, to a
change (of a few nanometres) in the absorption spectra of
the carotenoids in the membrane; this change results from the
effect on the carotenoids of the light-induced transmembrane
pmf (see PHOTOSYNTHESIS) and is sometimes referred to as an
electrochromic effect.
carotenoids A class of polyene (isoprenoid), aliphatic or alicyclic, commonly yellow or orange pigments; the class includes
the carotenes (hydrocarbons with usually nine conjugated double
bonds) and oxygen-containing derivatives of carotenes (xanthophylls) see figure. Carotenoids are widely distributed in
microorganisms, plants and animals; they are present in probably all photosynthetic organisms, in which they function e.g. in
LIGHT-HARVESTING COMPLEXES and in protecting CHLOROPHYLLS
from photodegradation. (See also SINGLET OXYGEN and ANTIOXIDANTS.) Carotenoids may also be involved in phototaxis (see
e.g. EYESPOT), and a carotenoid derivative, RETINAL, occurs in
certain bacterial energy-transducing systems (see PURPLE MEMBRANE). The presence of one or more particular carotenoids in
a given organism may be an important taxonomic feature, especially in algae.
Carotenes include e.g. b-carotene (R = R = b-ionone
ring, see figure), widely distributed in algae and higher
plants, and present in certain bacteria; a-carotene (an isomer
of b-carotene), also widely distributed; g-carotene (R = bionone ring, R = 2,6-dimethyl-1,5-heptadienyl), present e.g. in
some bacteria of the Chlorobiaceae; lycopene (R = R = 2,6dimethyl-1,5-heptadienyl), found e.g. in fruits.
Xanthophylls include e.g. antheraxanthin (found e.g. in
green algae (Chlorophyta), in chloromonads, and in plants);
astaxanthin (see PHAFFIA); BACTERIORUBERINS; diatoxanthin (in
cryptophytes); fucoxanthin (in brown algae (Phaeophyta), chrysophytes, diatoms and prymnesiophytes see figure); lutein
(3,3 -dihydroxy-a-carotene, common in plants and green algae);
myxoxanthophyll (a rhamnosyl-containing xanthophyll found in
cyanobacteria); neoxanthin (common in green algae and higher
plants); peridinin (in dinoflagellates); siphonein and siphonoxanthin (in siphonaceous green algae); spirilloxanthins (in anoxygenic photosynthetic bacteria); STAPHYLOXANTHIN; torularhodin
(in Rhodotorula); violaxanthin (in green algae and higher
plants); zeaxanthin (3,3 -dihydroxy-b-carotene, an isomer of
lutein, found e.g. in green algae and higher plants).
(See also MUTAGENICITY TEST.) Some apparent carcinogens actually require enzymic conversion within the body to an active
form, the ultimate carcinogen, before they can cause neoplastic
transformation.
(2) Syn. oncogen sensu lato (see ONCOGENIC).
carcinoma Any malignant tumour which arises from epithelial
tissue: see e.g. NASOPHARYNGEAL CARCINOMA and HEPATOCELLULAR CARCINOMA. (See also CANCER.)
cardiac beriberi See CITREOVIRIDIN.
Cardiobacterium A genus of oxidase-positive, catalase-negative,
Gram-negative bacteria which occur e.g. in the upper respiratory tract (see also HACEK) and which have been isolated from
the blood in cases of bacterial endocarditis. Cells: small, pleomorphic, non-motile, round-ended rods (0.50.75 13 m),
or filaments. Chemoorganotrophic. Aerobic and facultatively
anaerobic; apparently capnophilic. On anaerobic blood agar,
with 5% carbon dioxide, colonies are smooth and circular,
12 mm diam., after 48 hours. Strains are urease ve but
may be weakly indole +ve. Nitrates are not reduced. Optimum
growth temperature 3035 C. Media which have been used for
primary isolation include e.g. casein-soy broth and thioglycollate
broth (each containing SPS). No growth occurs on MacConkey
agar. Acid (but no gas) is formed from the fermentation of fructose, glucose, mannose, sorbitol or sucrose; lactic acid is the
main product of glucose fermentation. The organism is typically
sensitive to b-lactam and other antibiotics. GC%: 5962. Type
species: C. hominis.
cardioid condenser See MICROSCOPY (b).
cardiolipin Diphosphatidylglycerol. Such lipids occur e.g. in
bacterial CYTOPLASMIC MEMBRANES. Cardiolipin prepared by
alcoholic extraction of beef heart is used in STANDARD TESTS
FOR SYPHILLIS.
Cardiovirus A genus of viruses (family PICORNAVIRIDAE) isolated mainly from rodents; the true natural host is uncertain.
Cardiovirus virions are generally stable at pH 39, but are
labile at pH 4.56.4 in the presence of 0.1 M halide ions.
There is only one serotype, and the various named members of
the genus e.g. Columbia SK virus, mouse (or Maus) Elberfeld virus, mengovirus, MM virus are regarded as strains
of murine encephalomyocarditis virus (EMCV). EMCV causes
encephalitis and myocarditis in rodents, and a variant can cause
a diabetes-like syndrome in certain strains of mice [JGV (1985)
66 727732].
carfecillin See PENICILLINS.
caries (dental) See DENTAL CARIES.
cariogenic Refers to any factor, substance or organism which
promotes DENTAL CARIES.
carlaviruses (carnation latent virus group) A group of PLANT
VIRUSES in which the virions are slightly flexuous filaments (ca.
600700 13 nm) containing one molecule of linear, positivesense ssRNA (MWt ca. 2.7 106 ). Each member has a fairly
narrow host range, and some can cause disease in crop plants.
Transmission occurs (non-persistently) via aphids in at least
some members; mechanical transmission can be achieved under
experimental conditions. Type member: carnation latent virus.
Other members include e.g. cactus virus 2, hop latent virus,
HOP MOSAIC VIRUS, pea streak virus, potato virus M (= potato
paracrinkle virus), potato virus S, red clover vein mosaic virus.
Possible members include e.g. chicory blotch virus, eggplant mild
mottle virus, and groundnut crinkle virus.
CARNA See CUCUMOVIRUSES.
carnation etched ring virus See CAULIMOVIRUSES.
carnation Italian ringspot virus See TOMBUSVIRUSES.
128
(a)
R
R
(b)
O
HO
O C
CH3
(c)
C
O
HO
CAROTENOIDS. (a) General structure of a typical carotene. (b) b-Carotene (= b,b-carotene). (c) Fucoxanthin (a xanthophyll).
it is widely used in industry e.g. as a gelling and thickening agent in foods, pharmaceuticals etc, and in supports for
IMMOBILIZATION of cells and enzymes. It can also be used
as an AGAR substitute in certain bacteriological media [Book
ref. 2, pp. 144145]. The KCl-soluble, non-gelling fraction of
carrageenan consists of various polymers in which B = e.g.
D-galactose 6-sulphate, D-galactose 2,6-disulphate, 3,6-anhydroD-galactose 2-sulphate, etc. (The term l-carrageenan sometimes
refers to the whole KCl-soluble fraction, sometimes specifically
to the component in which A = D-galactose 2-sulphate, B = Dgalactose 2,6-disulphate.)
carragheen moss See CHONDRUS.
Carrel flask A squat cylindrical glass vessel which opens, at the
side, via a straight, upward-sloping tubular neck.
carrier (1) (med., vet.) An individual who harbours a particular
pathogen but shows no clinical signs of disease; such an individual can transmit the pathogen to others. Carriers are important
reservoirs of infection in certain diseases e.g. DIPHTHERIA and
TYPHOID FEVER (cf. SMALLPOX). [The carrier state (involving bacteria): JAC (1986) 18 Supplement A 181.] (2) (immunol.) See
HAPTEN. (3) See CARRIER TEST. (4) (virol.) See PSEUDOLYSOGENY
and CARRIER CULTURE.
carrier culture (virol.) A cell culture which is persistently
infected with a virus (see PERSISTENCE) but in which only a small
proportion of the cells in the population is actually infected by
the virus. The infected cells may release virus (e.g. by lysis)
but only a small proportion of the remaining cells is then
infected, and so on. The culture can be cured of the virus
e.g. by treatment with virus-neutralizing antiserum or by serial
subculture using small inocula. In e.g. mammalian cell cultures
a carrier culture may arise e.g. because INTERFERON production
may render most of the cells resistant to infection. (See also
PSEUDOLYSOGENY; cf. SEMIPERMISSIVE CELLS.)
carrier gene See FUSION PROTEIN.
carrier-specific T helper cell (CTh) A T LYMPHOCYTE whose
TCR recognizes a specific epitope in the carrier part of an
antigen another epitope (the hapten) on the same antigen
being recognized by a B cell. (See COGNATE HELP.) If an antigen
carrying a particular haptencarrier pair is used for primary
Some bacterial polyene pigments (e.g. FLEXIRUBINS, XANresemble carotenoids but lack the methyl groups
on the hydrocarbon chain.
(See also SPOROPOLLENIN.)
carp erythrodermatitis (Polish INFECTIOUS DROPSY) A FISH DISEASE affecting carp and certain other fish (e.g. goldfish, bream);
aetiology: unknown. The disease is subacute to chronic, with
variable mortality. Inflamed skin lesions become necrotic and
ulcerative, and generalized oedema follows. Secondary infection
with Aeromonas and Pseudomonas spp is common.
carp pox (epithelioma papulosum) A benign FISH DISEASE affecting the common carp (Cyprinus carpio) and other cyprinids.
Multiple transient hyperplastic nodules (up to several centimetres
across) develop on the skin and fins, and occasionally on the
eyes and gills; the lesions do not become necrotic. Carp pox is
apparently caused by a herpesvirus (see HERPESVIRIDAE).
carpomycetes Fungi which form fruiting bodies particularly
the ascomycetes and basidiomycetes.
Carr medium A medium used e.g. to distinguish between strains
of ACETOBACTER and GLUCONOBACTER; it contains yeast extract
(3%), agar (2%), BROMCRESOL GREEN (0.002%) and ethanol (2%
v/v). Gluconobacter strains (which typically oxidize ethanol to
acetic acid) produce colonies each surrounded by a yellow halo;
Acetobacter strains (which typically carry out overoxidation)
initially form similar colonies but, on further incubation, the
acetic acid is metabolized and the pH indicator reverts to its
original colour (i.e. the halo is lost).
carrageenan (carrageenin; carragheen) A mixture of sulphated
galactans associated with the CELL WALLS of many rhodophycean
algae (e.g. Chondrus crispus, Gigartina spp); they appear to
prevent desiccation when the alga is exposed to the atmosphere. Carrageenans have the general structure: -b-A-(1
4)-a-B-(1 3)-b-A-, where A = D-galactose 4-sulphate or Dgalactose 2-sulphate, and B is any of a range of sulphated
galactose or 3,6-anhydrogalactose residues. One component of
the carrageenan mixture, k-carrageenan, is precipitated by KCl;
in k-carrageenan A = D-galactose 4-sulphate, B = 3,6-anhydroD-galactose. k-Carrageenan forms gels with e.g. K+ , NH4 + ,
Ca2+ , Mg2+ , Fe3+ , and with water-miscible organic solvents;
THOMONADINS)
129
carrier test
forms in stationary-phase culture; on yeast extractglucose agar
the colonies are grey-white, pink or red. Up to 12% salt (NaCl)
can be tolerated. GC%: 6567. Type species: C. polymorphus.
caseous necrosis Syn. CASEATION.
caspases See APOPTOSIS.
cassava common mosaic virus See POTEXVIRUSES.
cassava latent virus See GEMINIVIRUSES.
cassava vein mosaic virus See CAULIMOVIRUSES.
cassette mechanism (mol. biol.) A system for gene regulation
in which a particular gene is removed from one site (active
slot), in which it can be expressed, to another (inactive slot)
in which it cannot be expressed another gene being inserted
into the active slot. (See e.g. MATING TYPE.)
Castanedas
method A form of BLOOD CULTURE in which the
catalase test
Among the bacteria there are several distinct mechanisms for
catabolite repression. Thus, e.g. one mechanism is characteristic
of E. coli and other enterobacteria, while others are typical
of AT-rich Gram-positive species (e.g. species of Clostridium,
Lactobacillus and Staphylococcus); each of these mechanisms is
regulated by signals from components of the PTS (q.v.). Models
outlining these mechanisms are described below.
(a) Catabolite repression in enterobacteria. In these organisms
the key regulatory molecule is the IIA component of glucose
permease in the PTS; note that, in this particular permease, IIA
is a cytoplasmic (i.e. soluble) protein.
When glucose is absent, phosphorylated IIA (IIAP) does
not undergo dephosphorylation via IIB, and under these conditions IIAP activates the enzyme ADENYLATE CYCLASE thus
stimulating the synthesis of CYCLIC AMP (cAMP). cAMP binds to,
and activates, the so-called cAMP-receptor protein (CRP) also
called catabolite activator protein, CAP, or catabolite gene activator protein, CGA protein. (CRP is encoded by the crp gene.)
The cAMPCRP complex acts as a transcriptional activator by
binding in the vicinity of promoters of certain operons (e.g.
lac), allowing them to be expressed in the presence of their
respective inducers. This explains why the inducibility of the
repressed operons can be at least partly restored by the addition
of cAMP. The precise way in which cAMPCRP promotes transcription is still unknown. One early model for the lac operon
supposed that the binding of cAMPCRP displaced RNA polymerase from a weak promoter, P2, to the primary promoter,
P1; that such a mechanism is unlikely to contribute significantly
to the transcription of the lac operon has been inferred from
the failure of inactivation of P2 to result in activation of P1
[Mol. Microbiol. (1992) 6 24192422]. Studies on e.g. the lac
operon suggest that the presence of cAMPCRP is not needed
after the establishment of a productive open complex, and that
only transient interaction is required between cAMPCRP and
RNA polymerase [EMBO (1998) 17 17591767].
When glucose (or other rapidly metabolizable substrate) is
present, unphosphorylated IIA binds to the permeases of various sugars (e.g. lactose), inhibiting uptake of the corresponding
sugars; as these sugars are involved in the induction of their
respective operons, this phenomenon is called INDUCER EXCLUSION.
Note that, in some cases, cAMPCRP may repress rather than
activate gene expression. For example, in Rhizobium meliloti
cAMPCRP blocks transcription of the dctA gene whose
expression is necessary for symbiotic nitrogen fixation [EMBO
(1998) 17 786796]. (In fact, CRP originally associated with
activation of catabolic operons is involved in a much wider
range of gene-regulatory activities.)
(b) Catabolite repression in the AT-rich Gram-positive bacteria. In these bacteria, transcription of some catabolic operons
is at least partly regulated by operon-specific regulator proteins,
each regulator protein having two phosphorylation sites; each
of these two sites is called a PRD (= PTS regulation domain).
PRDs can be phosphorylated by certain intermediates in the PTS
(IIBP and HPrP); one of the PRDs can be phosphorylated
by IIBP, the other by HPrP. It seems that phosphorylation
by IIBP is inhibitory, causing the regulator protein to inhibit
transcription from relevant operons, while phosphorylation by
HPrP promotes transcription from those operons. The activity of a given regulator protein thus depends on the mode of
its phosphorylation; thus, when phosphorylated only by HPr,
the regulator protein promotes transcription from all relevant
operons, but phosphorylation by HPr and IIB, or a lack of phosphorylation in both PRDs (i.e. in the presence of both inducer
and glucose), causes the regulator protein to function as a repressor of transcription. Induction of operon(s) therefore occurs only
under appropriate conditions, i.e. when (i) inducer is present and
(ii) glucose is absent. [PTS-dependent control of PRD-containing
regulators in induction and repression of catabolic operons: Mol.
Microbiol. (1998) 28 865874.]
A PRD-containing regulator protein in E. coli, BglG, is
involved in the control of the bgl operon (a b-glucoside catabolic
system concerned e.g. with the metabolism of salicin); in the
absence of b-glucoside, BglG is phosphorylated by the IIB
component of BglF (the b-glucoside permease) thus inhibiting
transcription of the bgl operon.
In AT-rich Gram-positive bacteria, catabolite repression
involving HPr and the enzyme HPr kinase occurs by ATPdependent phosphorylation of HPr at a site (Ser-46) which differs
from that (His-15) phosphorylated by enzyme I in the PTS; when
HPr is phosphorylated at Ser-46 it can form a complex with
catabolite control protein A (CcpA), and this complex can bind
to a regulatory site in target operons, inhibiting transcription.
(In vitro, phosphorylation of HPr at the Ser-46 site decreases
the ability of HPr to accept phosphate from the routine donor,
enzyme I; thus, phosphorylation of HPr at this site is likely to
inhibit uptake of sugars at the PTS permeases.) HPr kinase is
a bifunctional enzyme (HPr kinase/phosphatase), and its role
as a kinase in phosphorylating HPr under appropriate conditions of carbon availability is not fully understood; it is possible
that the kinase function of the enzyme is stimulated by fructose
1,6-bisphosphate (an intermediate in glucose catabolism). Inactivation of the HPr kinase gene (hprK ) in Staphylococcus xylosus
resulted in abolition of repression in the three catabolic enzyme
activities examined [JB (2000) 182 18951902].
catalase (H2 O2 :H2 O2 oxidoreductase; EC 1.11.1.6) A tetrameric
ENZYME, consisting of four ferriprotoporphyrin IX-containing
subunits, which catalyses the reaction 2H2 O2 2H2 O + O2 ;
with low concentrations of H2 O2 the enzyme can act as a
PEROXIDASE but this ability may not be common to catalases
from all sources [JGM (1983) 129 9971004]. Catalase plays a
vital role in detoxifying HYDROGEN PEROXIDE produced during
aerobic metabolism; it occurs in the majority of aerobic
organisms and is absent from most obligate anaerobes (though
present e.g. in Bacteroides fragilis). The enzyme is inhibited
by e.g. H2 S, HCN and N3 , and is inactivated by SUPEROXIDE.
Catalase is obtained commercially from e.g. Aspergillus niger
and Penicillium spp; it is used e.g. in the food industry for
removing excess H2 O2 (used for cold disinfection) from milk
and dairy products and from irradiated foods. (See also CATALASE
TEST; METHYLOTROPHY; PEROXISOMES; cf. PSEUDOCATALASE.)
catalase test A test commonly used with the object of determining whether or not a given bacterial strain produces CATALASE.
One drop of H2 O2 is added to a bacterial colony, or to a bacterial
emulsion; if the cells contain catalase, bubbles of gas (oxygen)
appear immediately or within one or two seconds. Such a (positive) reaction may indicate the presence of catalase or (e.g. in
some strains of Enterococcus faecalis) the presence of a PSEUDOCATALASE; certain bacteria can synthesize catalase only if they are
provided with haem. If, for the test, bacterial growth is obtained
from a blood-containing medium, care should be taken to prevent contact between H2 O2 and the medium: erythrocytes, which
contain catalase, can give rise to a false-positive reaction.
In carrying out the catalase test care should be taken to avoid
exposure to the AEROSOL produced by bursting bubbles; in one
method the test is carried out in a non-vented Petri dish: a drop
of H2 O2 and a speck of bacterial growth are placed at opposite
131
cataloguing
DISEASE; AUJESZKYS DISEASE; BOVINE EPHEMERAL FEVER; BOVINE
ULCERATIVE MAMMILLITIS; BOVINE VIRAL LEUKOSIS; BOVINE VIRUS
DIARRHOEA; CALF PNEUMONIA; FOOT AND MOUTH DISEASE; INFECTIOUS BOVINE RHINOTRACHEITIS; JEMBRANA DISEASE; LUMPY SKIN
DISEASE; MALIGNANT CATARRHAL FEVER; MUCOSAL DISEASE; PSEUDOCOWPOX; RABIES; RIFT VALLEY FEVER; RINDERPEST; ROTAVIRUS;
VESICULAR STOMATITIS. (e) Diseases of unknown/variable aetiology: ATYPICAL INTERSTITIAL PNEUMONIA; BOVINE RESPIRATORY
DISEASE; CALF SCOURS; WIMMERA GRASS POISONING; WINTER DYSENTERY.
(See also BOVINE SPONGIFORM ENCEPHALOPATHY.)
cattle plague Syn. RINDERPEST.
cattle tick fever Syn. REDWATER FEVER.
sides of the dish which, with the lid in place, is tilted so that the
H2 O2 runs onto the growth.
(See also SUPEROXOL TEST.)
cataloguing (of 16S rRNA) See RRNA OLIGONUCLEOTIDE CATALOGUING.
Catapyrenium A genus of LICHENS (order VERRUCARIALES) which
differ from DERMATOCARPON spp in having a squamulose thallus
attached to the substratum by rhizines. The genus includes e.g.
C. lachneum (formerly called e.g. Dermatocarpon hepaticum).
catarrh Inflammation of a mucous membrane, with excessive
production of mucus.
catecholamides (in iron uptake) See SIDEROPHORES.
catenane A complex of two or more circular nucleic acid
molecules interlocked like links in a chain. (cf. CATENATE;
CONCATEMER; see also GYRASE.)
Catenaria See BLASTOCLADIALES.
catenate (1) (verb) To interlock circular nucleic acid molecules
to form a CATENANE (hence noun catenation). (2) (adj.) Of e.g.
spores: formed in chains.
catenins See CADHERINS.
catheter-associated infection INFECTION (sense 3) associated
with catheterization of the blood vascular system or of the
urinary tract; in general, the risk of such infection increases
with the duration of catheterization. Catheter-related infections
account for a significant proportion of nosocomial disease.
In catheter-associated bacteraemia, the source of infection
can be investigated either with or without withdrawal of the
catheter [current methods for the diagnosis of catheter-related
bacteraemia: RMM (1997) 8 189195].
In catheter-associated infection of the urinary tract, a significant reduction in incidence during short-term (<3 weeks)
catheterization may be obtained by using catheters that have
anti-infection surface activity; such catheters may be either
(i) impregnated with e.g. nitrofurazone, or with minocycline
and rifampicin, or (ii) coated with a silver alloyhydrogel [EID
(2001) 7 342347].
cathodic depolarization theory A theory proposed to account
for the microbial corrosion of iron. In this theory, the spontaneous solubilization of iron (by ionization: Fe Fe2+ +
2e ) is promoted by (a) hydrogen formation, the electrons
from iron combining with protons derived from water ionization, and (b) utilization of the hydrogen by SULPHATE-REDUCING
BACTERIA. However, it has been reported that the primary
cause of such corrosion may involve an extracellular (probably phosphorus-containing) product of sulphate-reducing bacteria [Book ref. 155, pp. 619641].
cattle diseases Cattle may be affected by a wide range of diseases, some of which are specific to bovines; different species
and breeds of bovines may show differences in susceptibility to a given disease (see e.g. FOOT-ROT). (a) Bacterial diseases: see e.g. ACTINOMYCOSIS; ANAPLASMOSIS; ANTHRAX; BLACK
DISEASE; BLACKLEG; BRUCELLOSIS; CAMPYLOBACTERIOSIS; CONTAGIOUS BOVINE PLEUROPNEUMONIA; EPERYTHROZOONOSIS; FARCY
(sense 2); FOOT-ROT; HAEMORRHAGIC SEPTICEMIA (sense 2); INFECTIOUS KERATITIS; JOHNES DISEASE; LEPTOSPIROSIS; LISTERIOSIS;
MASTITIS; NECROBACILLOSIS; PARATYPHOID FEVER; RED WATER (of
calves); TUBERCULOSIS; TULARAEMIA; ULCERATIVE LYMPHANGITIS;
WHITE SCOURS. (See also COWDRIA; LAMZIEKTE; MIDLAND CATTLE
DISEASE.) (b) Fungal diseases: see e.g. ASPERGILLOSIS; ZYGOMYCOSIS. (See also FESCUE FOOT; 4-IPOMEANOL; PASPALUM STAGGERS;
PENITREMS; SPORIDESMINS.) (c) Protozoal diseases: see e.g. DALMENY DISEASE; EAST COAST FEVER; NAGANA; REDWATER FEVER.
(d) Viral diseases: see e.g. AKABANE VIRUS DISEASE; ALLERTON
Caulerpa
A genus of siphonaceous, tropical and subtropical
green seaweeds related to HALIMEDA (q.v.). The thallus consists
of a horizontal green rhizome with colourless rhizoids and erect
fronds. (See also ELYSIA.)
caulescent Becoming stalked or tailed.
cauliflower fungus Sparassis crispa.
cauliflower mosaic virus (CaMV; cabbage B virus) A member
of the CAULIMOVIRUSES which infects various brassicas. In
e.g. cauliflower (Brassica oleracea var. botrytis) symptoms of
infection typically include vein-banding and/or vein-clearing;
enations are occasionally formed. Transmission: chiefly styletborne via aphids.
A CaMV virion consists of a capsid (composed of a single
type of protein) and the dsDNA genome. In the virion, the
dsDNA is circular with three discontinuities at specific sites in
the molecule: two in one strand (the b strand), one in the other (a
strand); these discontinuities are neither nicks nor gaps, but are
sites of triple-stranded DNA in which the 3 and 5 ends overlap
by ca. 820 nucleotides [FEBS (1981) 134 6770]. In the host
plant, CaMV DNA appears to occur in the form of covalently
closed circular, supercoiled, histone-associated (chromatin-like)
mini-chromosomes which are apparently active in transcription
but not in replication. Only the a-strand is transcribed. Viral
RNAs (which are capped and polyadenylated) include a large
(8.2 kb, 35S) transcript corresponding to the length of the
entire genome with an additional 180-nucleotide terminal repeat;
this transcript may be an intermediate in DNA replication:
a molecule of plant tRNAmet binds to the 35S transcript at
a 14-bp region of homology, and this tRNA may act as a
primer for cDNA synthesis by reverse transcription (see RETROID
VIRUSES). [Evidence for replicative recombination in CaMV:
Virol. (1986) 150 463468.] Viral transcription occurs in the
plant cell nucleus, while virus particle assembly occurs in
rounded, amorphous, electron-dense, cytoplasmic viroplasms;
the site of DNA replication is unknown.
CaMV is widely studied as a model for transcription, DNA
replication etc in higher plants, and as a potential (nonintegrating) vector for gene transfer in plants.
[Book ref. 80, pp. 1748.]
caulimoviruses (cauliflower mosaic virus group) A group of
PLANT VIRUSES characterized by a dsDNA genome (ca. 8000 bp
long). The virions are isometric, ca. 50 nm diam.; the capsid
is composed of a single type of polypeptide (MWt ca. 42
103 ). Type member: CAULIFLOWER MOSAIC VIRUS; other members:
carnation etched ring virus, dahlia mosaic virus, figwort mosaic
virus, Mirabilis mosaic virus, strawberry vein-banding virus;
possible members: cassava vein mosaic virus, Petunia veinclearing virus, Plantago virus, thistle mottle virus. (See also
NON-CIRCULATIVE TRANSMISSION sense 1.)
Caulobacter A genus of chemoorganotrophic, strictly aerobic,
PROSTHECATE BACTERIA found e.g. in oligotrophic waters and in
132
CD8
soils poor in organic matter. Type species: C. vibrioides. GC%:
6467.
Most of the studies on this genus have been carried out on
C. crescentus to which the following account applies.
The non-motile, mature (mother) cell is a straight or curved
rod, ca. 12 m, which typically has a single polar stalk
(PROSTHECA) the distal end of which is adhesive; cells may
adhere, singly, to the substratum or may occur in groups
(rosettes), each group consisting of a number of cells radiating
from a central mass of adhesive material. Many strains contain
carotenoid pigments.
The mother cell gives rise, by asymmetric binary fission, to
a daughter cell (swarmer ) which bears a single polar flagellum.
The swarmer subsequently loses its flagellum, develops a
prostheca, and can then function as a mother cell. In stained
mother cells the prostheca may show one or more cross-striations
(crossbands), each of which is thought to mark one turn of the
cell cycle.
The molecular mechanisms involved in the process of differentiation and asymmetric cell division (essential features of
the cell cycle) are beginning to be understood through studies on the intracellular localization of proteins using techniques
such as gene fusion. In some cases the targeting, or activation,
of a specific protein has been linked to an essential aspect of
differentiation or cell division.
Cell cycle regulation involves various TWO-COMPONENT REGULATORY SYSTEMS. One response regulator, CtrA, has an important
role in the control of initiation of DNA replication and in the
expression of many genes [PNAS (2002) 99 46324637].
Following initiation of DNA replication in the mother cell,
levels of the phosphorylated form of CtrA (CtrAP) increase,
CtrAP (and/or CtrA) then promoting transcription of certain
genes including early flagellar genes and those regulatory
genes needed for expression of the later flagellar genes. The
regulation of flagellar genes may be more complex than was
previously supposed [PNAS (2002) 99 46324637].
The FliF protein is targeted to a specific polar site in
the developing daughter (swarmer) cell, i.e. the MS ring in
the swarmer cell develops prior to septation; the mechanism
responsible for directing FliF to the appropriate location is
unknown.
After formation of the septum, the FlbD protein is activated by
phosphorylation the kinase, FlbE, occurring near the septum
in the daughter cell; the activated FlbD protein (FlbDP)
promotes transcription of late flagellar genes resulting in the
development of a polar flagellum in the daughter cell.
In the daughter cell, CtrAP binds to the chromosomal origin,
thus inhibiting replication; hence, unlike the mother (stalked)
cell, the swarmer does not divide until it matures.
Under normal circumstances, the role of CtrA (i.e. the unphosphorylated form) in the mother cell includes activation of the late
cell division genes ftsQ and ftsA whose expression is necessary for cell division. If DNA replication is inhibited, then CtrA
is not synthesized (thus blocking cell division) lack of synthesis under these conditions reflecting failure of activation of ctrA;
as activation of ctrA is normally dependent on CtrAP, it has
been suggested that inhibition of DNA replication may inhibit
phosphorylation of CtrA constituting a cell cycle checkpoint
which blocks cell division in the absence of DNA replication
[EMBO (2000) 19 45034512].
[Control of differentiation in C. crescentus: Science (1997)
276 712718. Signal transduction mechanisms in C. crescentus
development and cell cycle control: FEMS Reviews (2000) 24
177191.]
CD11a/CD18
C4b components of complement, thus protecting the cell from
complement-mediated lysis.
The Sla antigen of the CR1 glycoprotein (an antigen of the
Knops blood group system) is associated with the phenomenon
of rosetting in falciparum MALARIA.
CD36 See MALARIA (vaccines).
CD40 A cell-surface molecule which occurs on B lymphocytes.
During recognition of a thymus-dependent (TD) antigen by
antigen-specific B and T cells, CD40 binds to the T cells
CD40L (gp39) antigen; such binding generates part of the
stimulus which results in clonal proliferation of the B cell and
class switching of antibody (IgM IgG etc.). (The physical
interaction between T and B cells also generates signals that
activate clonal proliferation in the T cell: see CD28.)
(See also RNA EDITING.)
CD41b See INTEGRINS.
CD44 (syn. homing-associated cell adhesion molecule, HCAM)
A CELL ADHESION MOLECULE found e.g. on monocytes, neutrophils, fibroblasts and memory T cells; it is apparently
unrelated to other CAMs. CD44 binds to e.g. collagen and
hyaluronate, and is apparently involved in lymphocyte homing (i.e. translocation of lymphocytes between blood and lymph
vessels).
CD46 (membrane co-factor protein, MCP) A cell-surface molecule on macrophages which acts as a receptor for COMPLEMENT
component C3b. (CD46 can also act as a receptor for the measles
virus; the binding of measles virus to CD46 inhibits the ability
of the macrophage to form INTERLEUKIN-12.)
CD48 A macrophage cell-surface glycoprotein which can bind
the type I FIMBRIAE of Escherichia coli. In the absence of
opsonizing factors, cells of E. coli that have type I fimbriae can
bind to CD48, initiating uptake into a phagosome which is not
acidified in the normal way and in which E. coli can survive.
CD50 See IMMUNOGLOBULIN SUPERFAMILY.
CD54 (syn. ICAM-1) A CELL ADHESION MOLECULE of the IMMUNOGLOBULIN SUPERFAMILY which occurs e.g. on endothelial and
epithelial cells, monocytes and fibroblasts. CD54 binds to certain
integrins (e.g. LFA-1, Mac-1). (See also INFLAMMATION.)
CD55 Decay-accelerating factor (DAF): a glycoprotein present in
the membranes of blood cells (red and white), endothelial cells,
and epithelial cells of the urinary and gastrointestinal tracts; DAF
accelerates decay of the C3 and C5 convertases in the classical
and alternative pathways of COMPLEMENT FIXATION, thus helping
to protect cells from complement-mediated lysis.
The DAF glycoprotein bears antigens of the Cromer blood
group system, and also acts as a receptor for Escherichia coli
and enteroviruses.
CD56 (syn. NCAM) See IMMUNOGLOBULIN SUPERFAMILY.
CD58 See IMMUNOGLOBULIN SUPERFAMILY.
CD61 See INTEGRINS.
CD62E (syn. E-selectin; also known as endotheliumleukocyte
adhesion molecule-1, ELAM-1) A CELL ADHESION MOLECULE
of the SELECTIN family which is inducible, on endothelial
cells, by certain cytokines (e.g. IL-1b, TNF-a); it binds to
sialylated carbohydrate ligands on e.g. monocytes, neutrophils
and CD4+ T cells. CD62E is involved in the tethering stage of
INFLAMMATION.
CD62L See SELECTINS.
CD62P See SELECTINS.
CD66 A category of cell adhesion molecules (of the
IMMUNOGLOBULIN SUPERFAMILY), some of which occur on
polymorphonuclear leukocytes (PMNs) and/or e.g. epithelial
cells. Specific molecule(s) CD66a, c, d and/or e (not b) can
celery yellows
critical level the concentration of initiator (per origin) then
falling sharply owing to the abrupt doubling of numbers of available origins at the start of replication. (It follows from this model
that a cell can govern its rate of division by regulating the rate
of synthesis of the initiator.)
In both models, initiation of DNA replication is a key event
which occurs late in an empirically defined phase that follows
cell division and precedes the next round of DNA replication.
Once DNA replication has begun the cell is normally committed
to continue replication to completion; the point at which a cell
becomes committed to DNA replication has been called the
restriction point (= R point, or R) or, simply, start.
(a) The eukaryotic cell cycle. The typical cell cycle in eukaryotes consists of the following sequence of phases:
S phase. DNA replication.
G2 phase. Gap phase 2: the period between the end of DNA
replication and the start of mitosis.
M phase. MITOSIS and cell division.
G1 phase. Gap phase 1: the period between cell division and
the start of DNA replication.
The total period (G1 + S + G2 ) is called interphase. (In some
lower eukaryotes, e.g. Physarum, the cell cycle apparently lacks
a G1 phase.)
Non-cycling (resting) cells are said to be in the G0 phase.
A given phase in the cell cycle is characterized e.g. by the
cells PLOIDY; thus, in a diploid cell, the ploidy is 2n in G1 ,
2n4n in S, and 4n in G2 .
Typically, when variation occurs in the rate of cell growth
and division (due e.g. to nutritional factors) it is the length of G1
which varies, i.e. the other two phases remain relatively constant
in length over a wide range of growth rates.
Regulation of the eukaryotic cell cycle. The cell cycle can be
regulated by signals from outside the cell; thus, cells exposed to
e.g. certain growth-inhibitory factors or sex pheromones become
arrested in the G1 phase. (Those cells which, at the time of
exposure, are in the S, G2 or M phase complete their cycling to
the G1 phase.)
To investigate regulatory mechanisms within the cell, studies
have been carried out e.g. on the yeasts Saccharomyces cerevisiae and Schizosaccharomyces pombe. Particularly useful have
been the cell-division-cycle mutants (cdc mutants) in which the
cell cycle is arrested at specific stage(s). The products of some
cdc genes have been found to influence more than one point
in the cycle; for example, the cdc2 gene product of S. pombe
(Cdc2) affects the cycle in late G1 and also in late G2 .
What kind of internal regulatory mechanisms are involved? At
certain points in the cell cycle there are gates or checkpoints
at which the cell makes a decision to either continue through the
cycle or stop cycling; one such checkpoint is start (mentioned
earlier). Continuation through start depends e.g. on the nutrient
status of the cells environment, i.e. the cycle is arrested at the
start checkpoint if nutrient levels are inadequate.
The effector molecules involved in regulating continue/stop
decisions are certain types of protein. They include PROTEIN
KINASES and PROTEIN PHOSPHATASES; a cyclical element is contributed by the CYCLINS (q.v.) which accumulate intracellularly,
prior to checkpoints, and are cleaved on passage through the
checkpoints.
(b) The prokaryotic cell cycle. In prokaryotes, most studies
on the cell cycle have been carried out on bacteria particularly
Escherichia coli ; the following account is based primarily on the
cell cycle in E. coli. [Cell cycle in the Archaea: Mol. Microbiol.
(1998) 29 955961.]
cell cycle
In bacteria, the cell cycle typically involves a period of growth
followed by division into two similar or identical daughter
cells (BINARY FISSION). (An atypical cell cycle occurs e.g. in
CAULOBACTER (q.v.).) The daughter cells receive equal numbers
of chromosome(s). Chromosome replication and cell division
are related in a manner described by the HELMSTETTERCOOPER
MODEL (q.v.).
The cells dimensions during growth. Cells that are growing
rapidly are larger (in both mass and volume) than those growing
more slowly. If the doubling time is less than 1 hour, the C
and D periods (see HELMSTETTERCOOPER MODEL) are more or
less constant; at the beginning of each C period the cells mass
(= initiation mass) is also virtually constant for a given rate of
growth. Under these conditions, it follows that the faster a cell
grows the greater will be the increase in cell mass and volume
during the (constant) C + D interval prior to cell division.
Cells of E. coli growing at a constant rate increase in size
mainly by elongation (the diameter of the cells remaining largely
unchanged). If the growth rate is increased, newly formed cells
are larger than those formed at the lower rate. During upregulation of the growth rate, the cells diameter increases
slowly, but the increase in cell length occurs more rapidly and, in
fact, initially overshoots cells being longer than appropriate
for the new, higher rate of growth; during ongoing growth at
the new rate, the cell diameter increases to its new value while
the cell length decreases to its final value (which is still higher
than that at the lower rate of growth). If growth rate falls, the
cells diameter, as before, adjusts more slowly than the cells
length the latter exhibiting an initial undershoot [JGM (1993)
139 27112714].
In Bacillus subtilis, determination of the rod shape appears
to involve helical, actin-like filaments within the cell. Filaments
composed of MreB protein may influence the cells width. Those
of Mbl protein influence longitudinal growth; they seem to guide
the cell-wall-synthesizing machinery. These types of protein are
found in many species, including Escherichia coli. Some bacteria
(e.g. Corynebacterium glutamicum) lack these proteins; in these
bacteria the rod shape may be maintained through polar growth.
[Bacterial morphogenesis: Cell (2003) 113 767776.]
Synthesis of the cell envelope. During steady growth, cell
envelope material is presumably being synthesized more or less
continually throughout the cell cycle. Studies on the turnover of
PEPTIDOGLYCAN in growing cells of the (Gram-negative) bacillus
E. coli suggest that the lateral wall of the cell contains a
monolayer of peptidoglycan and that multilayered peptidoglycan
may occur at the poles [JB (1993) 175 711]. In Gram-positive
bacteria, wall growth is believed to follow the INSIDE-TO-OUTSIDE
MODEL.
Holtje [Microbiology (1996) 142 19111918] described a
model for the mode of incorporation of newly synthesized
peptidoglycan in the growing sacculus: see THREE-FOR-ONE
MODEL.
It has been assumed that synthesis of the CYTOPLASMIC
MEMBRANE proceeds passively (secondarily to the growing
peptidoglycan sacculus). However, it has been reported that
peptidoglycan synthesis is dependent on the synthesis of membrane phospholipids a finding which suggests a novel mechanism for the regulation of growth of the cell envelope [Microbiology (1996) 142 28712877].
DNA replication. As mentioned, co-ordination between chromosome (DNA) replication and cell division is described by the
HELMSTETTERCOOPER MODEL.
Regulation of the initiation of a round of DNA replication is
not understood although a link between the timing of initiation
cell disruption
cycle, proteins are synthesized at the right times and targeted to
correct locations within the cell.
Control of the cell cycle. The occurrence of a given event
in the cell cycle could depend directly on the occurrence of
the previous event in the sequence. An alternative view is that
the cell cycle is a sequence of independent events that are coordinated. Co-ordination was suggested [Mol. Microbiol. (1991)
5 769774] for reasons that include e.g. (i) The inhibition of
certain cell cycle events does not necessarily inhibit others.
Thus, cell division can occur, for example, without proper
partitioning of the nucleoids i.e. division can proceed in the
absence of a signal from the event that normally precedes
division. (ii) There is no evidence for direct coupling between
chromosome replication and cell division. However, there is
evidence for indirect co-ordination: damage to DNA (which
may inhibit chromosome replication) triggers the so-called SOS
SYSTEM which, among other effects, inhibits cell division.
More recent studies on e.g. CAULOBACTER show that the cell
cycle has checkpoints: stages at which, normally, a given event
must be completed before the next can begin [see JB (2003) 185
11281146 (11351136)]. (See also essential TWO-COMPONENT
REGULATORY SYSTEMS.)
cell disruption The breaking of cells usually for analysis of
their components. Methods include: (a) Exposure to physical
forces (see e.g. BRAUN MSK TISSUE DISINTEGRATOR, FRENCH PRESS,
HUGHES PRESS, ULTRASONICATION). (b) Enzymic digestion of specific cell wall components e.g. the digestion of PEPTIDOGLYCAN by LYSOZYME or LYSOSTAPHIN; cells thus weakened can be
lysed osmotically. The morphology and structure of a cell influence the ease with which it is broken. Cells most resistant to
mechanical disruption include yeasts, bacterial endospores, and
Gram-positive cocci; Gram-negative bacteria are less resistant,
and the least resistant include protozoa and other animal cells.
Once cells are broken, their components become susceptible to
the action of e.g. AUTOLYSINS. (See also CELL FRACTIONATION.)
cell envelope (bacteriol.) The CYTOPLASMIC MEMBRANE together
with all layers external to it including the CELL WALL and/or
(where applicable) an S LAYER.
cell fractionation The separation of cell components. Fractionation is preceded by some form of CELL DISRUPTION. Methods
of fractionation include various forms of CENTRIFUGATION, CHROMATOGRAPHY and ELECTROPHORESIS.
cell-free ice nuclei See ICE NUCLEATION BACTERIA.
cell fusion See e.g. HYBRIDOMA; see also PROTOPLAST FUSION.
cell line (tissue culture) The heterogeneous population of cells
resulting from the first subculture of a PRIMARY CULTURE, or from
subsequent serial passaging of the cells. (cf. CLONED LINE and
ESTABLISHED CELL LINE.)
cell-mediated cytotoxicity Lysis of specific or non-specific target
cells by certain types of lymphoid cell. Lysis by CD8+ cytotoxic
T cells is triggered by specific antigen present at the surface
of the target cell, is subject to HISTOCOMPATIBILITY RESTRICTION
(involving MHC class I antigens), and is independent of both
antibody and complement (see T LYMPHOCYTE). Cytotoxicity
mediated by CD8+ T cells is important e.g. as a defence against
viral infections (antigen-specific T cells can lyse virus-infected
cells which bear virus-specific cell-surface antigens). Lysis of the
target cell requires a single collision with a functional cytotoxic
T cell which can kill repeatedly.
For other types of cell-mediated cytotoxicity see ADCC and NK
CELLS.
All types of cell-mediated cytotoxicity appear to require
divalent cations (Ca2+ , Mg2+ ).
cell wall
cell-mediated hypersensitivity Syn. DELAYED HYPERSENSITIVITY.
cell-mediated immunity (CMI) Any form of immunity which
can be transferred to a non-immune individual by the transfer of
cells (including e.g. LYMPHOCYTES) but not by (cell-free) serum
or plasma (see DELAYED HYPERSENSITIVITY), or in which cells are
directly involved as effectors (see CELL-MEDIATED CYTOTOXICITY).
(cf. HUMORAL IMMUNITY; see also AIDS.)
cell membrane Syn. CYTOPLASMIC MEMBRANE.
cell sap (1) The fluid in a plant cell vacuole. (2) Syn. CYTOSOL.
cell sorter See e.g. FACS.
cell wall In most algae, archaeans, bacteria and fungi: the structure which forms a (usually rigid) layer external to the CYTOPLASMIC MEMBRANE and which is responsible for the shape of
the organism; it protects the protoplast from mechanical damage, osmotic lysis etc., and it may also serve as a permeability
barrier to ANTIBIOTICS and other substances. Microbial cell walls
differ greatly in structure and composition, according to type
and species.
(a) Algal cell walls. Although a few algae (e.g. DUNALIELLA,
PORPHYRIDIUM) lack cell walls, the majority have a cell wall
composed of one or more layers of microfibrillar polysaccharide embedded in a matrix of amorphous polysaccharide (cf.
CHLAMYDOMONAS); in many species a layer of mucilaginous
polysaccharide also occurs external to the cell wall.
The most common microfibrillar component in algal cell walls
is CELLULOSE, which occurs e.g. in members of the Phaeophyta
and in many members of the Chlorophyta (e.g. Chaetomorpha, Chlorella, Scenedesmus), Rhodophyta and Xanthophyceae
(e.g. Botrydium, Vaucheria). The proportion of cellulose varies
from species to species but is often small compared with that
of the matrix polymers. In some green algae (e.g. Bryopsis (gametothallus), Caulerpa, Halimeda, Penicillus, Udotea)
and red algae (e.g. Palmaria palmata, Porphyra umbilicalis)
XYLANS replace cellulose as the main microfibrillar component
of the wall. A (1 4)-b-linked MANNAN is the main structural
polysaccharide in the cell walls of e.g. Acetabularia and Codium
spp; a mannan also occurs as an external layer (cuticle) in the
red algae Porphyra umbilicalis and Bangia fuscopurpurea. Xylomannan is a major component of Prasiola japonica.
Matrix polymers in algal cell walls are many and varied; they
include e.g. AGAR, ALGINATE, CARRAGEENAN and FUCOIDIN.
The walls of some algae contain inorganic materials such as
silica (see e.g. DIATOMS) and calcium carbonate (e.g. as a surface
encrustation in the CHAROPHYTES); calcium carbonate occurs as
calcite in some species, aragonite in others (e.g. HALIMEDA).
Many unicellular algae of the CHRYSOPHYTES, PRYMNESIOPHYCEAE
and PRASINOPHYCEAE have a cell covering composed of scales,
each consisting of an organic base in which silica or calcite may
be deposited. In the Prymnesiophyceae and Prasinophyceae
these scales are synthesized in the Golgi apparatus and are
released to the exterior by fusion of the Golgi vesicles with
the cytoplasmic membrane. (See also THECA.)
In those algae which have a heteromorphic alternation of generations, the different phases may have different cell wall structures/compositions; for example, in Derbesia marina/Halicystis
ovalis, the Derbesia phase has cell walls containing mannan,
while the Halicystis phase has walls containing cellulose and
glucoxylan. Gametes and spores may lack cell walls.
Many algal walls may be stained for light microscopy with
e.g. ALCIAN BLUE (for acidic polysaccharides), PAS, or TOLUIDINE
BLUE (which gives a pink colour with carboxyl and sulphate
groups).
[Review: Book ref. 38, pp 278332.]
cellar fungus
chitosan but no melanin, while spore walls of this fungus contain
much less chitosan, more glucan, and up to ca. 10% by dry
weight of MELANIN.
Wall structure also differs between mycelial and yeast forms
of DIMORPHIC FUNGI (sense 1); for example, in Mucor rouxii the
transition from mycelial form to yeast form is accompanied by
the appearance of mannan in the walls. In Paracoccidioides
brasiliensis the yeast-form walls contain (1 3)-a-D-glucan
as the sole glucan, while mycelial walls contain (1 3)-b-Dglucan/(1 6)-b-D-glucan in addition to the a-glucan.
In addition to their role as structural components, some
fungal wall polymers can be used as endogenous sources of
nutrient (for example, during carbon starvation or fruiting body
formation see e.g. PSEUDONIGERAN).
Certain antifungal antibiotics function by interfering with
cell wall biosynthesis: see e.g. ACULEACIN A; NIKKOMYCINS;
PAPULACANDIN B; POLYOXINS.
(See also GROWTH (fungal).)
(d) Archaeal cell walls. Distinctive types of cell wall occur in
members of the Archaea; there are also wall-less species (e.g.
Thermoplasma).
Archaeal walls include those which consist mainly or solely
of an S LAYER that is closely associated with the cytoplasmic
membrane; this type of wall occurs e.g. in species of Desulfurococcus, Halobacterium, Methanococcus and Thermoproteus.
Heteropolysaccharides occur in the cell walls of Halococcus and
Methanosarcina, and PSEUDOMUREIN occurs in the cell wall of
Methanobacterium and Methanobrevibacter.
cellar fungus Coniophora puteana. (cf. WET ROT.)
cellobiase See CELLULASES.
cellobiohydrolase Exoglucanase: see CELLULASES.
cellobiose A reducing disaccharide: b-D-glucopyranosyl-(1
4)-D-glucopyranose. (See also CELLULASES and LIGNIN.)
cellobiose:quinone oxidoreductase See LIGNIN.
cellodextrins Oligomers of (1 4)-b-D-linked glucopyranosyl
residues formed by the action of CELLULASES on CELLULOSE.
cellular (1) Of or pertaining to a cell or cells. (2) Having the
form and characteristics of a (single) cell. (3) Composed of
two or more cells. (cf. ACELLULAR; see also UNICELLULAR and
MULTICELLULAR.)
cellular immunity (1) CELL-MEDIATED IMMUNITY. (2) Aspects of
NON-SPECIFIC IMMUNITY mediated e.g. by macrophages and other
phagocytic cells.
cellular microbiology A branch of microbiology concerned with
the interactions between microorganisms and eukaryotic cells at
the molecular level. [Science (1996) 271 315316; Book ref.
218.]
cellular slime moulds SLIME MOULDS in which the vegetative
phase consists of uninucleate amoeboid cells (myxamoebae)
which aggregate to form a multicellular pseudoplasmodium from
which the fruiting bodies arise. Classes: ACRASIOMYCETES and
DICTYOSTELIOMYCETES. (cf. MYXOMYCETES.)
cellulases Enzymes which degrade at least some forms of CELLULOSE. Endoglucanase (endo-(1 4)-b-D-glucanase, endocellulase, (1 4)-b-D-glucan 4-glucanhydrolase, EC 3.2.1.4) attacks
more or less randomly at sites within (1 4)-b-D-glucan chains
in amorphous regions of cellulose or at the surfaces of microfibrils. Exoglucanase (exo-(1 4)-b-D-glucanase, exocellulase,
(1 4)-b-D-glucan cellobiohydrolase, EC 3.2.1.91) releases
cellobiose (and, in some cases, glucose) from non-reducing ends
of b-D-glucan chains. b-Glucosidase (cellobiase, b-D-glucoside
glucohydrolase, EC 3.2.1.21), hydrolyses cellobiose and watersoluble cellodextrins to glucose. Many cellulolytic organisms
produce a number of isoenzymes.
cellulose
Isolated microbial cellulases have relatively low specific
activities and are costly to obtain; they currently have only
limited commercial use. Pilot schemes include the use of
cellulases or cellulolytic organisms for the saccharification of the
cellulose in waste materials such as straw, sugarcane bagasse,
sawdust, newspaper etc (see e.g. INDUSTRIAL ALCOHOL and
SINGLE-CELL PROTEIN). (See also ENZYMES.)
(See also PAPER SPOILAGE.)
cellulin granules Granules, composed of CHITIN and (1 3)-band (1 6)-b-linked glucan, found in the cells of fungi of the
LEPTOMITALES; the granules are composed of alternating concentric
layers of chitin and glucan. (cf. CONCENTRIC BODIES.)
cellulitis A diffuse, spreading, inflammatory condition affecting
(usually) subcutaneous tissues and characterized by oedema,
redness and pain. Common causal agents are streptococci and
staphylococci. Orbital cellulitis (inflammation of the eye-socket)
may be caused by Haemophilus influenzae. (See also ERYSIPELAS
and GAS GANGRENE.)
cellulolytic Able to degrade CELLULOSE.
Cellulomonas
A genus of aerobic or facultatively anaerobic,
asporogenous bacteria (order ACTINOMYCETALES, wall type VIII)
which occur e.g. in soil. In young cultures the organisms are
slender, irregular rods (diam. ca. 0.50.6 m) and/or filaments,
with or without primary branching, but shorter rods and/or
coccoid forms occur in the stationary phase; the cells are
Gram-positive, but easily decolorized, and cells which are
apparently Gram-negative may predominate. The organisms are
non-motile, or motile by one to several polar flagella [IJSB
(1984) 34 218219]. Growth occurs e.g. on peptone meat
extract at 30 C; all strains require biotin and thiamine for
growth. Typically, a yellow non-diffusible pigment is formed
when growth occurs on nutrient agar. Glucose is metabolized to
acid both oxidatively and fermentatively. Cellulomonas spp are
amylolytic and cellulolytic (see CELLULASES). Species include
C. biazotea, C. cellasea, C. flavigena, C. fimi, C. gelida, and
C. uda. GC%: 7177. Type species: C. flavigena.
cellulose A linear (1 4)-b-D-glucan. Cellulose occurs in plants
(it is the main structural component of the cell walls in most
plants), in the CELL WALLS of most algae and certain fungi, in
certain cellular slime moulds (e.g. in the sheath surrounding
the sorocarp stalk, in the spore walls, and in the slime of
migrating slugs of Dictyostelium discoideum), and in the cyst
walls of Acanthamoeba spp; extracellular cellulose is produced
by certain bacteria: e.g. Acetobacter xylinum (see PELLICLE
sense 1), Sarcina ventriculi (most strains of which form a
cellulose microcapsule apparently responsible for the formation
of the characteristic packets of cells), strains of Agrobacterium
and Rhizobium (in which extracellular cellulose is involved in
the adhesion of bacteria to plants), and various floc-forming
bacteria in activated sludge.
Native cellulose occurs largely in the form of (crystalline)
microfibrils (a-cellulose) each composed of stacked sheets
of parallel, hydrogen-bonded glucan chains. Each chain is in
extended form (held rigid by intrachain hydrogen bonds) and
contains many glucosyl residues (e.g. 200015000, depending
on source). In plant cell walls the microfibrils are embedded in a
matrix of HEMICELLULOSES, LIGNIN and PECTIC POLYSACCHARIDES;
regions of amorphous cellulose, infiltrated with hemicelluloses,
also occur. [Plant cell wall structure: Book ref. 38, pp. 946.]
Cellulose may be stained for microscopy e.g. with CONGO RED
or CALCOFLUOR WHITE both of which also inhibit microfibril
formation during cellulose synthesis. [Biosynthesis of cellulose
in microorganisms: Book ref. 62, pp. 85127.]
cellulosome
The strength of a centrifugal field (at a given point) is
given by:
4p2 (revs min1 )2 r
G=
3600
h
Ra
9
loge
2 !2 r2p (rp r)
Rb
cephalodium
sample is layered onto a density gradient column, and centrifugation is continued until equilibrium is reached, i.e., each particle
has reached that part of the gradient which corresponds to its
own density (its isopycnic or equal density position). Particles
in a heterogeneous sample are thus separated on the basis of
their individual densities: particles of different density can be
separated even if they are similar in size and shape.
Rate-zonal centrifugation (also called band, gradient differential, s zonal, zonal, or zone centrifugation). The sample is
layered onto a density gradient column, and centrifugation is
continued until the various types of particle in the sample form
layers or bands at different levels within the column at which
time centrifugation is stopped. The separation of particles into
bands is thus achieved on the basis of the differing sedimentation
rates of the particles.
Ultracentrifugation is used e.g. for the sedimentation of
macromolecules, for the determination of molecular weights, for
purifying plasmid DNA, for characterizing viruses, and as an
indirect method for estimating the GC% of bacterial DNA. The
principles involved are similar to those given earlier in the entry;
however, while the common laboratory centrifuge can develop
a maximum field of ca. 5000 to 10000 g, the ultracentrifuge can
achieve fields of the order of 500000 g. In an ultracentrifuge
the rotor is housed in a refrigerated and evacuated chamber,
and the instrument incorporates various optical systems (e.g.
the SCHLIEREN SYSTEM) and photographic systems so that the
progress of sedimentation can be followed and recorded at all
times. (See also SVEDBERG UNIT.)
If a species of DNA is subjected to isopycnic ultracentrifugation in a caesium chloride gradient, the DNA forms a band at a
region of the gradient corresponding to its buoyant density (Bd);
the Bd of e.g. chromosomal DNA from Escherichia coli is ca.
1.7 g/cm3 . Since there is a linear relationship between Bd and
GC%, the value of Bd can be used for estimating GC% (q.v.).
Ultracentrifugation can also be used to separate cccDNA
(e.g. plasmid DNA) from linear DNA or from circular, nicked
DNA (e.g. nicked chromosomal DNA). cccDNA can incorporate
smaller amounts of certain INTERCALATING AGENTS (e.g. ETHIDIUM
BROMIDE) than can equivalent molecules of the other forms of
DNA. The incorporation of e.g. ethidium bromide decreases the
Bd of the DNA molecule. Thus, if e.g. a plasmid-containing
bacterial lysate is centrifuged in a caesium chlorideethidium
bromide gradient, cccDNA may form a distinct band of higher
Bd; such a procedure has been called dyebuoyant density
centrifugation.
centriolar plaque Syn. SPINDLE POLE BODY.
centriole In many types of eukaryotic cell: an intracellular
microtubular structure (see MICROTUBULES) which is involved in
some types of MITOSIS and which, in some cells, can develop into
a BASAL BODY; centrioles do not occur in e.g. some types of fungi.
Essentially, a centriole is a hollow cylinder, ca. 300400 nm
in length, whose wall is formed of 9 longitudinally arranged
triplets of microtubules; one end of the cylinder contains a dense
intracentriolar material. The structure appears to lack DNA, but
RNA may be present. A centriole is often surrounded by a
number of dense pericentriolar structures which, collectively,
are sometimes referred to as a centrosome and which can
act as a MICROTUBULE-ORGANIZING CENTRE. (Centrosome is
also used to refer to the entire structure, i.e., centriole(s) plus
pericentriolar structures.) Centrioles are often formed from preexisting centrioles, but they can also be formed de novo.
Centrohelida An order of protozoa (class HELIOZOEA) in which
the cell typically has an eccentric nucleus and a central body
cephaloridine
or different morphotypes (phycosymbiodemes) of the same
mycobiont. [Chimeroid associations in Peltigera: Lichenol.
(1978) 10 157170.]
cephaloridine See CEPHALOSPORINS.
cephalosporin C See CEPHALOSPORINS.
cephalosporin N Syn. PENICILLIN N.
cephalosporin P1 A steroid antibiotic structurally related to
FUSIDIC ACID.
cephalosporinase A b-LACTAMASE active mainly or solely
against CEPHALOSPORINS.
cephalosporins A class of antibiotics each characterized by a
molecular structure which includes a b-lactam ring fused to a
dihydrothiazine ring (see b-LACTAM ANTIBIOTICS for structure and
mode of action). (cf. CEPHALOSPORIN P1 and PENICILLIN N.)
Cephalosporin C (the first to be prepared) is produced e.g.
by Acremonium kiliense (= Cephalosporium acremonium); this
antibiotic has poor antibacterial activity.
A range of semi-synthetic cephalosporins can be prepared
from the 7-aminocephalosporanic acid (7-ACA) derivative of
cephalosporin C. When introduced, the earlier cephalosporins
(collectively) had useful activity against a range of bacteria,
and were typically (particularly cefotaxime and cefuroxime)
less susceptible than PENICILLINS to b-LACTAMASES; moreover,
compared to penicillins, cephalosporins were found to be less
frequently allergenic.
When introduced, the first- to third-generation cephalosporins
were characterized by antibacterial spectra such as: mainly
Gram-positive (cephalexin, cephaloridine); good activity against
Gram-positive and moderate activity against b-lactamasenegative Gram-negative species (cephalothin); Gram-positive
species and e.g. Neisseria gonorrhoeae and Haemophilus
influenzae (cefuroxime); limited spectrum, but some activity
against Pseudomonas aeruginosa (cefsulodin); Gram-negative
species, including Haemophilus influenzae (cefotaxime). (Note
that cephalosporins (and e.g. the cephamycin CEFOXITIN)
have little or no activity against enterococci.) The earlier
cephalosporins (and some of the newer ones) are commonly
susceptible to extended-spectrum b-LACTAMASES (q.v.). (See also
CEPHAMYCINS.)
Some cephalosporins can be administered orally, while others
(e.g. cefuroxime, cefotaxime) are administered parenterally.
First-generation cephalosporins include e.g. cefazolin,
cephalexin, cephaloridine and cephalothin.
Second-generation cephalosporins include e.g. cefamandole,
cefonicid [Drugs (1986) 32 222259], ceforanide, cefsulodin
and cefuroxime.
Third-generation cephalosporins include e.g. cefixime, cefmenoxime [Am. J. Med. (1984) 77 (supplement 6A)], cefotaxime, ceftazidime [Am. J. Med. (1985) 79 (supplement 2A)],
ceftizoxime and ceftriaxone.
Fourth-generation cephalosporins include e.g. CEFEPIME and
cefpirome.
(Note. In the literature, the names of some cephalosporins are
spelt with either f or ph.)
Cephalosporium See ACREMONIUM. (For C. lecanii see VERTICILLIUM.)
Cephalothamnium A genus of colonial CHRYSOPHYTES in which
a cluster of biflagellate, non-pigmented cells extends from the
tip of a single stalk.
cephalothin See CEPHALOSPORINS.
cephamycins Antibiotics (7-a-methoxyCEPHALOSPORINS) produced by Streptomyces spp or prepared from cephalosporins.
Compared with those cephalosporins which lack the 7-amethoxy group, cephamycins (e.g. CEFOXITIN) tend to have
decreased antibacterial activity but increased resistance to bLACTAMASES and improved penetrability of the Gram-negative
outer membrane.
cephems Compounds which contain the cephalosporin nucleus
(see b-LACTAM ANTIBIOTICS). (cf. OXACEPHEMS.)
cephradine See CEPHALOSPORINS.
Ceraceosorus See BRACHYBASIDIALES.
ceramide See SPHINGOMYELIN.
Ceramium See RHODOPHYTA
Ceratiomyxa A genus of SLIME MOULDS formerly classified with
the acellular slime moulds (MYXOMYCETES); currently, the genus
is placed e.g. in a separate class, Ceratiomyxomycetes, of the
MYXOMYCOTA, or in zoological schemes is classified with the
protostelids e.g. in the subclass Protosteliia (see EUMYCETOZOEA).
C. fruitculosa is a widespread and common species found e.g.
on bark and rotting wood. The vegetative PLASMODIUM is almost
hyaline. Prior to fruiting, it produces copious amounts of a
mucoid matrix, and plasmodium and matrix become extended
to form upright, usually branched white columns (110 mm
tall) which solidify on drying; sporocarps develop on the surface
of these columns, each sporocarp consisting of a long slender
stalk bearing a single round or cylindrical spore. The spores are
deciduous. On germination of a spore, a quadrinucleate thread
stage is produced, and this eventually gives rise to 4, then
8, flagellated haploid cells which can apparently function as
gametes; a diploid vegetative plasmodium develops from the
zygote formed by fusion of two of these flagellated cells.
Ceratiomyxella See PROTOSTELIOMYCETES.
Ceratiomyxomycetes See CERATIOMYXA.
Ceratium
A genus of DINOFLAGELLATES in which the cells
typically bear 3 or 4 horn-like thecal extensions: one arising
from the epicone, 2 or 3 from the hypocone.
Ceratobasidiaceae See TULASNELLALES.
Ceratobasidium See TULASNELLALES.
Ceratocystis A genus of fungi (order OPHIOSTOMATALES) which
include various plant pathogens see e.g. DUTCH ELM DISEASE
and OAK WILT. (See also BLUE STAIN, PINE DISEASES, and IPOMEAMARONE.)
C. ulmi forms erumpent perithecia (see also ASCOSPORE), and
in the imperfect (Pesotum) state can form individual conidia on
simple conidiophores or chains of conidia in a drop of mucus at
the tip of a dark, bristle-like synnema (ca. 1 mm high).
C. coerulescens forms superficial perithecia, and in the
Chalara state can form cylindrical or ellipsoidal conidia.
Ceratomyces See LABOULBENIALES.
Ceratomyxa See MYXOSPOREA.
Cercophora See SORDARIALES.
cercopithecine herpesvirus 1 See B VIRUS.
Cercospora
A genus of fungi (class HYPHOMYCETES) which
include many plant-pathogenic species e.g. C. beticola (causal
agent of leaf spot of beet), and C. apii (e.g. on celery). The
organisms form septate mycelium; conidia are characteristically
thread-like and multiseptate.
cereal chlorotic mottle virus See RHABDOVIRIDAE.
cereal diseases Diseases of members of the Gramineae cultivated
for their edible grain. Some of the common diseases are listed
below. Although some diseases are specific to particular types
of cereal, others can also affect certain wild grasses; thus, e.g.
the causal agents of HALO SPOT and LEAF BLOTCH can both grow
on cocksfoot (Dactylis glomerata) and Timothy grass (Phleum
pratense). (See also GRASS DISEASES.)
Barley. See e.g. BROWN RUST, ERGOT, EYESPOT (sense 2),
GLUME BLOTCH, HALO SPOT, LEAF BLOTCH (rhynchosporium), NET
144
Chagas disease
H+ -ATPase
see also
CF0 F1
See PROTON ATPASE.
CFA/I, CFA/II See ETEC.
CFP-10 See ESAT-6.
CFT COMPLEMENT-FIXATION TEST.
cfu Colony-forming unit: see COUNTING METHODS.
CGA protein See CATABOLITE REPRESSION.
CGB agar Canavanine-glycine-bromthymol blue agar: a medium
used to distinguish between certain strains of CRYPTOCOCCUS.
On this medium, C. neoformans var. gattii hydrolyses glycine,
raising the pH and causing the BROMTHYMOL BLUE to turn blue;
the few strains of C. neoformans var. neoformans which can
hydrolyse glycine are inhibited by the L-canavanine. [Recipe
and method: Book ref. 100, p. 95.]
CH region See IMMUNOGLOBULINS.
CH50 See HD50
Chaenotheca See CALICIALES.
Chaetoceros
A large genus of planktonic centric DIATOMS in
which the cells are often joined together by long setae.
Chaetocladium See MUCORALES.
Chaetomella See SPHAEROPSIDALES.
Chaetomium A genus of fungi (order SORDARIALES) which form
evanescent asci in perithecia which bear long, curved, coiled
and/or branched hairs or bristles; the unicellular, commonly
dark ascospores are discharged from the perithecium in a
gelatinous mass. Most or all species are strongly cellulolytic
(see CELLULASES, PAPER SPOILAGE, SOFT ROT (sense 1), TEXTILE
SPOILAGE). (See also COMPOSTING and OLIVE-GREEN MOULD.)
Chaetomorpha A genus of unbranched, filamentous, siphonocladous green algae (division CHLOROPHYTA).
Chaetophora A genus of uniseriate, filamentous (heterotrichous)
green algae (division CHLOROPHYTA) which occur in freshwater
habitats, usually attached to rocks, plants etc. Long colourless
multicellular hairs extend from the ends of the (branched) filaments. Quadriflagellate zoospores and biflagellate isogametes are
formed. Related genera include e.g. Draparnaldia, Fritschiella,
STIGEOCLONIUM and URONEMA.
chaga fungus The sterile fruiting body of Inonotus obliquus.
Chagas disease An acute or chronic, often fatal, systemic
TRYPANOSOMIASIS of man which occurs in Central and South
America. The causal agent, Trypanosoma (SCHIZOTRYPANUM)
cruzi, is typically transmitted contaminatively by blood-sucking
TRIATOMINE BUGS (family Reduviidae): metacyclic forms in the
bugs faeces infect via wounds, abrasions and mucosal surfaces.
(The pathogen can also be transmitted by blood transfusion and,
via the milk, to breast-fed infants. Transplacental transmission
occurs in over 1% of cases in endemic areas.) Reservoirs of bugtransmissible pathogens exist in domestic animals (e.g. dogs) and
wild animals (e.g. anteaters, armadillos, opossums, certain rats
and primates). [Book ref. 72, pp 161182.]
In the patient, T. (S.) cruzi occurs as non-dividing trypomastigotes in the blood, and in the reproductive amastigote and
epimastigote forms in pseudocysts within host cells. Symptoms
may include cardiomyopathy, grossly enlarged colon (megacolon) and oesophagus, and low levels of certain hormones
resulting from damage to endocrine glands. Autoantibodies to
heart and skeletal muscles, and to nerve tissue, have been
detected. Lab. diagnosis: microscopical examination of thick
blood films; XENODIAGNOSIS (using e.g. Dipetalogaster maxima); a CFT and/or e.g. immunofluorescence tests. Treatment:
chemotherapeutic agents, e.g. Lampit (a nitrofuran) and benznidazole (a 2-nitroimidazole), are commonly used but are associated with significant side-effects; moreover, this treatment may
or may not eliminate the intracellular forms of T. (S.) cruzi.
LUTEOVIRUSES
145
chain-termination method
a nascent protein either co-translationally [JBC (1997) 272
3271532718] or following translation.
Although most chaperones are proteins, a membrane lipid acts
as a chaperone for the LacY protein in Escherichia coli [EMBO
(1998) 17 52555264].
Chara See CHAROPHYTES.
Charales See CHAROPHYTES.
charcoal blood agar A medium used for the primary isolation of
Bordetella pertussis; it is reported to yield better growth than that
obtained with the traditional BORDETGENGOU AGAR. Beef extract,
starch, peptone, NaCl, nicotinic acid and agar are dissolved in
water by heating; charcoal is added before autoclaving. Sterile,
defibrinated horse blood is added to the molten agar at 45 C.
[Recipe: Book ref. 219, pp 470, 471.]
CharcotLeyden crystals Microscopic, colourless crystals often
present in the stools of patients suffering from certain intestinal
diseases (e.g. amoebic dysentery) or in the sputum of patients
with asthma or other chest conditions. The crystals are diamondshaped or shaped like short, double-pointed needles; they stain
with iodine.
charge-shift immunoelectrophoresis IMMUNOELECTROPHORESIS
used e.g. to distinguish amphiphilic from hydrophilic proteins.
Differentiation is based on the fact that when amphiphilic
proteins bind non-ionic detergent at their hydrophobic sites, their
electrophoretic mobility is changed by the addition of (positively
or negatively charged) ionic detergent; hydrophilic proteins are
unaffected.
chargerin See ANISOTROPIC INHIBITOR.
Charon A type of CLONING vector derived from the genome of
bacteriophage l; typically, a Charon is a REPLACEMENT VECTOR.
charonin An ATP-dependent protease which may also function
as a molecular chaperone.
Charophyceae See CHLOROPHYTA.
Charophyta See CHAROPHYTES.
charophytes A group of macroscopic green algae variously
regarded as (a) a distinct division (Charophyta) [e.g. Book
ref. 123, pp. 303330]; (b) a class (Charophyceae) within the
division Chlorophyta [e.g. Book ref. 130, pp. 36132]; or (c) an
order (Charales) within a class, Charophyceae, which is broader
than that in (b): see CHLOROPHYTA. Charophytes (e.g. Chara
and Nitella) have several features in common with bryophytes
(mosses and liverworts): e.g., the plant is structurally complex,
being differentiated into root-, shoot- and leaf-like structures;
the shoots are divided into nodes (each node bearing a whorl
of branches) and internodes; sexual reproduction is oogamous,
and an envelope of sterile cells (shield cells) surrounds the
antheridia and oogonia; asexual reproduction may occur e.g.
by the formation of bulbils (plantlets) on the rhizoids, or
of AMYLUM STARS on the lower nodes, but apparently never
by the formation of zoospores. Charophytes are generally
heavily calcified (hence the popular names stoneworts or
brittleworts); they occur mainly in fresh water (lakes, ponds,
etc). (See also GYROGONITES.)
chasmoendolith See ENDOLITHIC.
Chattonella See CHLOROMONADS.
chauveolysin See THIOL-ACTIVATED CYTOLYSINS.
che gene In e.g. enterobacteria: a gene involved in CHEMOTAXIS.
checker colony See DRAUGHTSMAN COLONY.
Cheddar cheese See CHEESE-MAKING.
cheese-making Cheese is made by the coagulation and fermentation of MILK; differences between the various types of cheese
reflect differences in e.g. mode of manufacture, microorganisms
employed, and type of milk used (e.g. cows, goats sheeps).
Dinitroaniline herbicides such as trifluralin (a,a,a-trifluoro2,6-dinitro-N,N-dipropyltoluidine), which inhibit certain protozoan parasites by affecting tubulin polymerization, have been
examined for their potential as candidate antimicrobials against
T. cruzi [TIP (2001) 17 136141].
[The disease in Mexico: TIP (2001) 17 372376.]
chain-termination method (of DNA sequencing) See DNA SEQUENCING.
Chainia See STREPTOMYCES.
Chalara See HYPHOMYCETES and CERATOCYSTIS; see also MURAMIDASE.
chalcomycin See MACROLIDE ANTIBIOTICS.
chalk-brood A BEE DISEASE caused by Ascosphaera apis. Infected
honey-bee larvae become fluffy and swollen, and later shrink and
harden; death usually occurs after the larvae have been sealed in
their cells. Some of the dead larvae remain chalky-white, others
become dark-coloured. Infection occurs by ingestion of spores
of A. apis. The spores germinate in the gut; mycelium develops
in the gut lumen and penetrates the gut wall. Fruiting bodies
may form on the outside of the larvae.
Ascosphaera spp can also cause chalk-brood in wild bees
e.g. A. aggregata in the alfalfa leaf-cutting bee Megachile rotundata [life cycle of A. aggregata: Mycol. (1984) 76
830842].
challenge (immunol.) The exposure of an animal (or other living
system) to a pathogen (or other agent) usually in order to
determine the state of immunity or resistance to the pathogen
or agent; for example, an animal may be challenged with
a pathogen to test the efficacy of a previously administered
vaccine.
challenge virus See INTERFERENCE (1).
chalybeate (of water) Containing iron.
Chamaesiphon A genus of unicellular CYANOBACTERIA (section I)
in which the cells are ovoid and reproduce by repeated budding
at the apical end; the buds were formerly known as exospores.
GC%: ca. 47.
Chamaesiphonales See CYANOBACTERIA.
Chamberland candle See FILTRATION.
chamois contagious ecthyma virus See PARAPOXVIRUS.
champagne See WINE-MAKING.
chancre A papular lesion formed at the initial site of infection
in certain diseases (e.g. SYPHILIS, SLEEPING SICKNESS).
chancroid (soft chancre) A VENEREAL DISEASE, caused by
Haemophilus ducreyi, characterized by one or more ulcerative
lesions which are usually confined to the genitalia. Incubation
period: 114 (usually 45) days.
Changuinola subgroup See ORBIVIRUS.
channel catfish virus disease (CCVD) A FISH DISEASE which
affects cultivated channel catfish (Ictalurus punctatus) under
4 months of age. Symptoms include e.g. abnormal swimming
movements, haemorrhages of gills, skin and internal organs,
and necrotic lesions in liver, spleen etc. The causal agent is
a herpesvirus (see HERPESVIRIDAE).
chanterelle See CANTHARELLALES.
Chaos
A genus of large, multinucleate, freshwater amoebae
of the AMOEBIDA [Book ref. 133, p. 145]. In C. carolinense
polypodial forms may be 0.72.0 mm in diam., monopodial
forms up to 3 mm diam.; C. illinoisense is generally smaller
(ca. 0.51.5 mm).
chaperone (molecular chaperone) In most cases: a protein that is
specialized for folding/stabilization or direction of a (typically
newly synthesized) protein. (See also HEAT-SHOCK PROTEINS,
FIMBRIAE (type I) and VIRULON.) A chaperone may bind to
146
chemiluminescence
has been made of a starter culture containing organisms that
produce the BACTERIOCIN lacticin 3147 which inhibits Listeria
monocytogenes [JAM (1999) 86 251256]. Cream cheese (for
example, Neufchatel ) is made in a similar way using cream
instead of skim milk; it thus has a higher fat and lower moisture
content.
(f) Mozzarella is a soft, usually unripened, Italian cheese
formerly made from buffalo milk (but now generally made from
cows milk). Its manufacture is similar to that of Cheddar but
involves higher temperatures (5055 C) as well as thermophilic
streptococci and lactobacilli.
(g) Parmesan is a hard, low-moisture Italian cheese; its
manufacture is similar to that of Swiss cheeses (see below),
but e.g. propionibacteria are not used.
(h) Swiss cheeses (e.g. Emmentaler, Gruy`ere) are manufactured in a way basically similar to that used for Cheddar; however, the process involves higher cooking temperatures
(5055 C) and uses thermophilic bacteria (Streptococcus thermophilus, Lactobacillus spp). Strains of Propionibacterium are
used in the inoculum; during ripening, these bacteria (i) contribute flavour components (e.g. propionic acid), and (ii) produce
carbon dioxide which collects in pockets, thus forming the
characteristic eyes in the cheese.
(See also CHEESE SPOILAGE and DAIRY PRODUCTS.)
cheese spoilage High-moisture cheeses (e.g. cottage cheese)
are very susceptible to spoilage by a wide range of bacteria
and moulds, while low-moisture cheeses (e.g. parmesan) are
much more resistant. Surface spoilage of cheeses is commonly
due to the growth of moulds e.g. species of Aspergillus,
Cladosporium and Penicillium, and (in high-moisture cheeses)
Geotrichum spp. Bacteria may produce off-flavours e.g. H2 S
(produced e.g. by clostridia), rancidity (due e.g. to lipolytic
pseudomonads); undesirable holes (eyes) may be formed
during the ripening process by gas-producing bacteria (e.g.
coliforms, Bacillus spp).
cheese-washers lung An EXTRINSIC ALLERGIC ALVEOLITIS associated with the inhalation of allergens from Penicillium spp e.g.
P. verrucosum (P. casei ).
CHEF See PFGE.
chelating agents See e.g. CDTA, EDTA, EGTA, NTA.
chemical shift See NUCLEAR MAGNETIC RESONANCE.
Chemiclave An apparatus used e.g. for sterilizing surgical instruments etc; essentially, it consists of a chamber within which
instruments etc are exposed to a mixture of the vapours of alcohol, formaldehyde and water at 132 C, 20 lb/inch2 (ca. 137 kPa).
(cf. AUTOCLAVE.)
chemiluminescence The production of light as a result of a
chemical reaction. The term is commonly used to refer e.g.
to the emission of light by phagocytes and other specialized
mammalian cells under appropriate conditions, and to light emission in cell-free experimental systems, while BIOLUMINESCENCE
usually refers to the emission of light from whole, living organisms; in all cases the emission of light is O2 -dependent. In those
cases where the mechanism is known, light emission involves the
oxidation of a particular type of organic molecule the resulting unstable, excited molecule spontaneously returning to the
(unexcited) ground state with concomitant emission of light. (cf.
PHOSPHORESCENCE.) Chemiluminescence in phagocytes is associated with the respiratory burst which occurs in e.g. NEUTROPHILS
during PHAGOCYTOSIS.
Experimental chemiluminescence systems employ lightemitting substances such as lucigenin (bis-N-methylacridinium
nitrate), lophine (2,4,5-triphenylimidazole) and LUMINOL.
147
chemiluminogenic probe
the matrix side of the inner membrane which becomes relatively
alkaline and electrically negative. By contrast, in the chloroplast
thylakoid membrane, protons are pumped inwards during PHOTOSYNTHESIS, so that electrochemical gradients develop in the
opposite orientation.
Respiring cells of Escherichia coli develop a pmf of the
order of 200 mV; thus, e.g. 1y may be ca. 100 mV and 1pH
ca. 1.75 (1p = 205 mV). These cells maintain an internal
pH of ca. 7.47.8 when the extracellular pH ranges from 5.5
to 9.0, i.e., the bulk-phase transmembrane 1pH is highly
dependent on the extracellular pH. (By contrast, in Clostridium
pasteurianum a decrease in extracellular pH from 7.1 to 5.1
corresponds to a decrease in internal pH from 7.5 to 5.9 [Book
ref. 82, pp. 137138].) In respiring E. coli, the 1p drops sharply
if the external pH rises above ca. 7.8, though 1p can be
augmented under these conditions by increasing the extracellular
concentration of K+ or Na+ [JB (1985) 163 423429]. In
chloroplasts, the contribution of 1pH to 1p is typically much
greater than it is in bacteria such as E. coli.
In a respiring bacterial cell there is a characteristic proton
circuit: protons are extruded across the cytoplasmic membrane
by the primary pmf generator (electron transport chain) and they
re-cross the membrane via an H+ -ATPase during ATP synthesis.
In such a cell the pmf acts as a thermodynamic back-pressure
which opposes further extrusion of protons. However, proton
extrusion can occur not only through the operation of an electron
transport chain: it can also occur as a result of the tendency of the
intracellular reaction (ATP ADP + Pi) to reach equilibrium;
in a respiring cell, the energy derived from metabolism holds
this reaction far to the left of its equilibrium position, so that the
tendency to reach equilibrium (by ATP hydrolysis) is associated
with a large amount of Gibbs free energy (1GATP ; 1Gp ;
phosphate potential ; phosphorylation potential ). 1GATP tends
to promote ATP hydrolysis (at the H+ -ATPase on the inner side
of the membrane) and, hence, to promote proton extrusion in
opposition to the pmf. 1GATP and pmf may tend to maintain
a dynamic balance; however, if pmf is below a certain value
ATPases tend to become (reversibly) inactivated: see PROTON
ATPASE. Pmf is the primary factor responsible for RESPIRATORY
CONTROL.
Experimental manipulation of 1p, 1y or 1pH . Various
IONOPHORES can be used to collapse or modify pmf or either
of its components. Thus, e.g., VALINOMYCIN can alter 1y,
without altering 1pH, by permitting K+ influx into the bacterial
cytoplasm sufficient to reduce or eliminate 1y. By contrast,
NIGERICIN can effect an electroneutral exchange of K+ for
H+ , thus altering 1pH without disturbing 1y. UNCOUPLING
AGENTS can abolish 1p (or prevent its development) and (as
a consequence) can abolish respiratory control. Other agents
(e.g. AUROVERTINS, DCCD, efrapeptin, OLIGOMYCIN, QUERCETIN,
TENTOXIN and tributyltin chloride) can inhibit (F0 F1 )-type H+ ATPases.
Measurement of 1p. The components of 1p (1y and 1pH)
are estimated separately and added.
1y is often estimated by allowing an indicator ion to
distribute across the membrane so as to reach electrochemical
equilibrium with the membrane potential; at equilibrium, a
measurement is made of the concentration of the indicator ion
on either side of the membrane, and 1y is estimated from
the Nernst equation (see equation 3 in ION TRANSPORT). The
indicator ion must be permeable only by electrical uniport
(so that its equilibrium distribution reflects 1y); it should
not be bound or metabolized; it should disturb the membrane
(1)
chemotaxis
attractant for e.g. fibroblasts) and IP10 (produced by monocytes
and endothelial cells, attractant for e.g. NK cells). (The two
latter chemokines are reported to have anti-angiogenic activity,
and they may inhibit tumour formation.)
Chemokines of the CC family include eotaxin (produced
by macrophages and endothelial cells, attractant primarily for
eosinophils) and RANTES (regulated on activation, normal T
cell expressed and secreted: produced by T cells, monocytes
and epithelial cells, attractant for e.g. T cells and NK cells).
Chemokines of the C family include lymphotactin: a (murine)
protein produced e.g. by activated T cells and a potent attractant
for T cells.
chemoklinokinesis Klinokinesis (see KINESIS sense 2) in which
the stimulus is a change in concentration of a chemical.
chemolithoautotroph A CHEMOTROPH with properties of a LITHOTROPH and an AUTOTROPH. The ability to grow chemolithoautotrophically is confined to a relatively small number of
prokaryotes; these organisms make important contributions to the
cycles of matter, and some are involved in LEACHING processes.
Plasmid-mediated anaerobic chemolithoautotrophic growth
has been reported for a strain of Sulfolobus ambivalens containing the plasmid pSL10. Aerobically, this organism derives
energy from the oxidation of elemental sulphur (with oxygen as
the terminal electron acceptor), yielding sulphuric acid; anaerobically it obtains energy from the oxidation of hydrogen (with
elemental sulphur as terminal electron acceptor), yielding hydrogen sulphide [Nature (1985) 313 789791].
chemolithoheterotroph A CHEMOTROPH with the properties of a
LITHOTROPH and a HETEROTROPH. (See also MIXOTROPHY.)
chemolithotroph See CHEMOTROPH.
chemoorganoheterotroph A CHEMOTROPH with the properties of
an ORGANOTROPH and a HETEROTROPH. The majority of bacteria
and fungi are chemoorganoheterotrophs (cf. CHEMOLITHOAUTOTROPH); some such bacteria are facultative chemolithoautotrophs. Taken together, chemoorganoheterotrophs can use a
very wide range of organic substrates, though particular species
may be able to use only a very limited number of compounds. Because most if not all chemoorganotrophs are
heterotrophic, the term heterotroph is sometimes used as a
synonym of chemoorganoheterotroph.
chemoorganotroph See CHEMOTROPH.
chemoprophylaxis The use of drug(s) for PROPHYLAXIS.
chemoreceptor See CHEMOTAXIS.
chemorepellent See CHEMOTAXIS.
chemorespiration See PHOTORESPIRATION.
chemostat See CONTINUOUS CULTURE.
chemosynthetic primary production See PRIMARY PRODUCTION.
chemotaxigen Any agent which promotes the formation of a
CYTOTAXIN.
chemotaxis A TAXIS in which the stimulus is a concentration gradient of a given chemical (a chemoeffector). A cell may make
a net movement towards higher concentrations of some chemoeffectors (chemoattractants) but away from others (chemorepellents); a chemoattractant may or may not be a nutrient. Cells may
exhibit chemotaxis when they occupy a physiologically suboptimal position within the concentration gradient.
A cell capable of chemotaxis must be able to (i) detect
(sense) changes in the concentration of a chemoeffector,
(ii) transmit this information to locomotory organelle(s), and
(iii) make the appropriate response; it must also be able to
adapt by resuming the unbiased mode of motility when in a
uniform concentration of chemoeffector, regardless of the actual
concentration.
chemotaxis
of chemoattractant it will exhibit a greater tendency to tumble
(clockwise flagellar rotation) thus increasing the probability of
changing to a more favourable direction.
Sensing the concentration gradient is achieved by means
of specific receptors (in the cytoplasmic membrane) to which
the chemoeffector binds; the binding of chemoeffector to a
receptor results in the transmission of a signal that promotes
either counterclockwise or clockwise flagellar rotation that is,
either smooth swimming or tumbling, respectively.
MOTILITY
chemoeffector
periplasm
(a)
MCP
CM
cytoplasm
signal
chemoeffector
(b)
MCP
ATP
+CH3
CH3
CheW CheA
ADP
CheR
CheB
CheY- P
CW
P
CheZ
low
(c)
high
high
Cattr
Cattr
low
low
MCP
M
CCW
(smooth)
CW
(tumble)
150
chemotaxis
maltose complex binds to the Tar protein, and the galactose
and ribose complexes bind to the Trg protein. (Uptake and
metabolism of these sugars are not necessary for a chemotactic
response.)
Cells can also respond chemotactically to substrates taken
up by PTS (q.v.). The mechanism is not understood, but one
suggestion is that particular PTS component(s) interact via
unknown intermediate(s) with the CheY protein (see figure),
thus influencing flagellar rotation. PTS-mediated chemotaxis
differs from the MCP system in several ways e.g. (i) substrates
must be transported, not simply bound; (ii) adaptation does not
involve methylation; and (iii) the system does not respond to
repellents [e.g. JCB (1993) 51 16].
The mechanism by which flagellar rotation is switched
between counterclockwise and clockwise modes appears to be
independent of pmf, although pmf is necessary for driving the
flagellar motors (cf. AEROTAXIS and PHOTOTAXIS).
Interestingly, although SWARMING in E. coli involves components of the chemotaxis system, the substances that promote
swarming appear to differ from the known chemoeffectors in
chemotaxis [PNAS (1998) 95 25682573].
151
chemotaxonomy
can be transmitted e.g. by hyphal anastomosis; no capsid has
been detected (cf. MYCOVIRUS), but the dsRNA appears to be
closely associated with an RNA polymerase and may be packaged within vesicles formed by the host fungus [JGV (1985)
66 26052614]. [Potential of the hypovirulence factor for biological control of E. parasitica: ARPpath. (1982) 20 349362;
Science (1982) 215 466471.] (See also DUTCH ELM DISEASE.)
chi site (chi sequence) See RECBC PATHWAY.
chi structure See RECOMBINATION.
c1776 A disabled strain of Escherichia coli K12 which e.g.
requires various amino acids (including diaminopimelic acid)
and is highly sensitive to bile salts and other detergents. It was
constructed for use in CLONING experiments to reduce the risk of
propagation of potentially dangerous clones should they escape
from the laboratory. However, c1776 is difficult to grow and to
transform, and is currently rarely used.
chiasma The visible manifestation of CROSSING OVER e.g.
between non-sister chromatids of homologous chromosomes
during MEIOSIS.
chiasma interference See INTERFERENCE (sense 2).
chiastobasidial Refers to a transverse arrangement of nuclear
spindles in a developing BASIDIUM. (cf. STICHOBASIDIAL.)
chick embryo lethal orphan virus See AVIADENOVIRUS.
ChickMartin test A SUSPENSION TEST used to determine the
PHENOL COEFFICIENT of a (phenolic) disinfectant; it assesses the
efficacy of a disinfectant in the presence of organic matter,
i.e., under conditions more closely approximating those in
practical use (cf. RIDEALWALKER TEST). (Many disinfectants are
inactivated by organic matter.) In the original test the organic
matter used was 3% sterile dry faeces; a modified form of the
test uses a sterilized suspension of yeast (5% dry wt/vol.). To
each of several serial dilutions of the disinfectant under test
are added the yeast and an inoculum of Salmonella typhi. After
incubation for 30 min, an inoculum from each dilution is added
to each of two tubes of broth which, after incubation at 37 C
for 2 days, are examined for growth. The same procedure is
carried out with phenol. For the phenol test two dilutions are
identified: (i) that containing the highest concentration of phenol
which permitted growth in both tubes inoculated from it, and
(ii) that containing the lowest concentration of phenol which did
not permit growth in either tube inoculated from it; the mean
of these two concentrations is then calculated (Pmean ). For the
disinfectant under test Dmean is calculated in the same way. The
phenol coefficient of the disinfectant is given by Pmean /Dmean .
chicken diseases See POULTRY DISEASES.
chicken syncytial virus See AVIAN RETICULOENDOTHELOSIS VIRUSES.
chickenpox (varicella) An acute, highly infectious disease which
usually occurs in epidemics affecting mainly young children.
The causal agent is human (alpha) herpesvirus 3 (varicellazoster virus) see ALPHAHERPESVIRINAE. Infection occurs by
direct contact or by droplet inhalation. The incubation period
is ca. 23 weeks. Symptoms: fever and a rash of erythematous
macules which rapidly develop into thin-walled vesicles, finally
becoming dry and crusty; successive crops of lesions occur. The
disease is usually mild and self-limiting; complications include
e.g. pneumonia (usually in adults), encephalitis, and secondary
infection of skin lesions with staphylococci and streptococci.
In immunosuppressed or CMI-defective patients the disease is
much more severe, with extensive rash and severe systemic
symptoms (progressive varicella) which may be fatal; vidarabine
and acyclovir have been used in treatment. A live vaccine has
been developed [MS (1985) 2 249254]. Lab. diagnosis: viruses
Chl
in arthropod exoskeletons, in the CELL WALLS of most fungi,
in certain algae (e.g. in the spines of many planktonic centric
diatoms and in the lorica of Poterioochromonas stipitata see
OCHROMONAS), and in certain protozoa (e.g. in the cyst walls of
ciliates and amoebae); it is apparently never formed by bacteria.
Native chitin occurs in the form of microfibrils in which
extended glucan chains are hydrogen-bonded together (antiparallel in a-chitin, parallel in b-chitin) to form sheets which, in turn,
associate (by hydrogen-bonding in a-chitin but not in b-chitin)
to form microfibrils.
Biosynthesis of chitin involves the enzyme chitin synthase (EC 2.4.1.16) which catalyses the polymerization of Nacetylglucosamine from UDP-N-acetylglucosamine precursors.
The enzyme requires Mg2+ or Mn2+ and phospholipids for
activity, and is inhibited e.g. by POLYOXINS and NIKKOMYCINS.
The location of chitin synthase in fungal cells is controversial;
most reports suggest that it occurs in the cytoplasmic membrane [Book ref. 38, pp. 403405], while evidence has been
presented that it is mainly cytoplasmic in Mucor rouxii [JGM
(1984) 130 11931199]. (See also CHITOSOME and GAMMA PARTICLE (sense 2).) Chitin synthase occurs in zymogen and active
forms; its activity in the cell may be controlled by regulation
of the proteolytic activation of the zymogen at sites of chitin
synthesis. [Chitin biosynthesis in microorganisms: Book ref. 62,
pp. 85127.] (See also GROWTH (fungal).)
(See also CHITINASE.)
chitinase (poly-[1,4-b-(2-acetamido-2-deoxy-D-glucoside)] glycanohydrolase; EC 3.2.1.14) An enzyme which degrades CHITIN
to chitobiose [JGM (1984) 130 18571861]; chitobiose can
be hydrolysed to N-acetylglucosamine by chitobiase (N-acetylb-D-glucosaminidase, EC 3.2.1.30). Chitinases are produced
by a wide range of organisms: e.g., chitin-containing fungi;
microorganisms parasitic on chitin-containing organisms (e.g.
entomopathogens see also BURNED SPOT DISEASE); insectivorous animals (e.g. spiders); and plant tissues (where they may
play a role in resistance to fungal diseases [Nature (1986) 324
365367]).
chitinolytic (chitinoclastic) CHITIN-degrading: see CHITINASE.
chitobiase See CHITINASE.
chitobiose A disaccharide consisting of two (1 4)-b-linked Nacetyl-D-glucosamine residues.
chitosan (mycosin) A polymer of non-acetylated (1 4)-blinked D-glucosamine residues (cf. CHITIN). It occurs in nature as
a CELL WALL constituent in the hyphae of certain zygomycetes
(e.g. Mucor spp) and as a minor component of the spores of
Fusarium solani (in which it is a strong elicitor of PHYTOALEXIN production by pea plants [Book ref. 58, pp. 270271]).
[Coordination of chitosan and chitin synthesis: JGM (1984) 130
20952102.]
chitosome A type of vesicular particle (4070 nm diam.) comprising a membrane-like shell containing chitin synthase; chitosomes can be isolated from a wide range of fungi and can
synthesize CHITIN microfibrils from UDP-N-acetylglucosamine
in vitro. Initially, coiled microfibrils develop within the chitosome which then apparently breaks open to release extended
microfibrils. It is uncertain whether chitosomes are organelles
(serving e.g. in the transport of chitin synthase from its site of
synthesis to its site of action) or small vesiculated fragments of
cytoplasmic membrane formed during the isolation procedure.
Chitin synthase can be released from chitosomes by treatment
with digitonin.
Chl Chlorophyll: see CHLOROPHYLLS.
Chlamydia
infection the cycle is complete each infected host cell containing ca. 101000 EBs in an inclusion which may occupy a major
part of the cell. On release, EBs infect fresh host cells.
Antibiotic resistance. Chlamydiae are typically sensitive to
e.g. tetracyclines. Penicillins may inhibit the development of
EBs from RBs, although the mechanism of such inhibition
is unknown. Most strains of C. trachomatis are sensitive to
sulphonamides.
C. pecorum. A species from ruminants (including sheep
and cattle) which can cause e.g. respiratory, intestinal and
neurological disease. [Description of C. pecorum: IJSB (1992)
42 306308.]
C. pneumoniae. A species first isolated from a suspected
case of trachoma in Taiwan (strain TW-183) and subsequently
from a case of acute respiratory infection (strain AR-39). These
organisms, initially thought to be strains of C. psittaci, were
referred to as TWAR strains [see Book ref. 193, pp 321340]
but later classified in a new species, C. pneumoniae [description
of C. pneumoniae: IJSB (1989) 39 8890]. [Phylogenetic relationship of C. pneumoniae to C. psittaci and C. trachomatis:
IJSB (1993) 43 610612.] C. pneumoniae is associated with
e.g. epidemics of subacute respiratory disease; re-infection, or
chronic infection, can lead to severe disease, apparently involving immunologically-based pathogenesis.
C. psittaci. Hosts: commonly birds and mammals other than
man (but see PSITTACOSIS); C. psittaci appears to have played
a significant role in an epizootic of urogenital and respiratorytract disease and keratoconjunctivitis in the koala (Phascolarctos
cinereus) [AJEBMS (1985) 63 283286]. Folic acid and
glycogen are not formed.
C. trachomatis. Natural hosts: man and mouse; no strains have
been isolated from birds. Folic acid and glycogen are formed.
Three biovars: trachoma (typically non-invasive, confined almost
exclusively to squamocolumnar epithelial cells), lymphogranuloma venereum (LGV) (typically invasive, infects e.g. lymph
nodes), and mouse (isolated only from mice; has an affinity
for the lungs). Biovars trachoma and LGV can be distinguished
(by means of microimmunofluorescence tests) by virtue of their
type-specific antigens: AK and L1 L3 , respectively. [Complete
genome sequence: Science (1998) 282 754759.]
Chlamydiaceae See CHLAMYDIALES.
Chlamydiales An order of Gram-negative bacteria which are
obligate intracellular parasites in eukaryotic cells; the organisms
multiply within cytoplasmic vacuoles and exhibit a developmental cycle which includes small, rigid-walled infectious forms
(elementary bodies), and larger, non-infectious forms (reticulate bodies, sometimes called initial bodies) which have flexible
walls and which divide by fission. One family, Chlamydiaceae,
which comprises a single genus, CHLAMYDIA.
Chlamydodon See HYPOSTOMATIA.
Chlamydomonas A large genus (>500 species) of unicellular,
usually flagellated green algae (division CHLOROPHYTA cf. PHYTOMASTIGOPHOREA) which are widespread and common in a
range of freshwater habitats and e.g. on damp soils. (See also RED
SNOW.) The vegetative cells are usually pyriform or ovoid, ca.
520 m in length, uninucleate, haploid, and usually motile by
means of two similar flagella which project from the anterior end
(cf. PALMELLOID PHASE). (See also FLAGELLUM (b) and FLAGELLAR
MOTILITY (b).) The cell wall is thin and contains no cellulose,
being composed of a complex of hydroxyproline-rich glycoproteins [wall structure: JCB (1985) 101 15501568, 15991607].
The cell contains a single large CHLOROPLAST which may be
cup-shaped, stellate, H-shaped, lobed, etc, according to species.
chlorguanide
and also made synthetically. Chloramphenicol is a broadspectrum bacteriostatic agent active against a wide range of
bacteria; it also inhibits vegetative growth and sporulation in
certain fungi [JGM (1983) 129 34013410].
Chloramphenicol binds to the 50S subunit of prokaryotic and
mitochondrial RIBOSOMES (but apparently not to the ribosomes in
at least some archaeans [SAAM (1985) 6 125131]); it inhibits
peptidyltransferase and, hence, PROTEIN SYNTHESIS.
Resistance to chloramphenicol in bacteria is commonly
due to a plasmid-specified enzyme chloramphenicol acetyltransferase (CAT; also called chloramphenicol transacetylase) which catalyses an acetyl-CoA-dependent acetylation of
chloramphenicol at the C-3 hydroxy group to form a compound
with little or no antibiotic activity. Plasmid-specified CAT is
usually or always synthesized constitutively in Gram-negative
bacteria but inducibly (see also TRANSLATIONAL ATTENUATION) in
e.g. staphylococci and streptococci. (See also Tn9.)
CAT-producing bacteria can be detected by rosanilin dyes [JB
(1982) 150 13751382].
Non-enzymic resistance to chloramphenicol may be due e.g.
to (mutant) ribosomes which fail to bind the antibiotic. Pseudomonas aeruginosa is innately resistant, being able normally to
tolerate high levels of the drug.
Chloramphenicol antagonizes those antibiotics (e.g. penicillins) which inhibit only actively growing and dividing bacteria. Its clinical usage is limited by its toxicity.
chloranil (tetrachloro-p-benzoquinone) A QUINONE ANTIFUNGAL
AGENT used e.g. as a seed dressing for the prevention of damping
off, seed rots etc; it decomposes in the presence of light.
chlorazol black E A black amphoteric triazo DYE used e.g. for
the VITAL STAINING of Mycoplasma spp and L-forms [JB (1969)
99 17].
chlorbutanol (chlorbutol) Trichloro-t-butanol; it is used e.g. as
a PRESERVATIVE (at ca. 0.5% w/v) in ophthalmic solutions. At
room temperatures chlorbutanol is unstable at alkaline pH, and it
can be inactivated by colloids such as bentonite and magnesium
trisilicate.
chlorbutol Syn. CHLORBUTANOL.
Chlorella A genus of non-motile, unicellular green algae (division CHLOROPHYTA) which occur in fresh water, on soils, bark
etc, and in association with various other organisms (see
ZOOCHLORELLAE). (cf. VAMPIROVIBRIO.) The cells are spherical
(ca. 215 m diam.); each contains a single haploid nucleus
and a large, usually cup-shaped chloroplast with or without a
pyrenoid. The CELL.WALL contains cellulose and e.g. SPOROPOLLENIN. Asexual reproduction occurs by AUTOSPORE formation:
the protoplast divides to form 2, 4, 8 or 16 daughter protoplasts
which develop cell walls before being released by rupture of the
parent wall. Motile cells are never formed. (cf. CHLOROCOCCUM.)
The paucity of morphological features in Chlorella spp has
led to an increased use of chemotaxonomy in this genus [Book
ref. 123, pp. 391407]. Although primarily photosynthetic,
some Chlorella spp can ferment glucose to lactate under
anaerobic conditions. Most species can reduce NO3 , and a
few can produce extracellular gelatin- and/or starch-hydrolysing
enzymes.
(cf. PROTOTHECA; see also SINGLE-CELL PROTEIN and YAKULT.)
chlorguanide (Paludrine; proguanil) N 1 -p-chlorophenyl-N 5 -isopropyldiguanide: an antimalarial drug (see MALARIA) which,
itself, has little activity but which is converted in vivo to a
highly active cyclic form (cycloguanil a substituted dihydrotriazine). Cycloguanil binds competitively to the enzyme
dihydrofolate reductase (DHFR), inhibiting the synthesis of
tetrahydrofolate.
chlorhexidine
larvae and purified virus pellets exhibit a yellow-green
iridescence. Virions (ca. 180 nm diam.) are ether-resistant. Type
species: mosquito iridescent virus; other members include insect
iridescent viruses 35, 7, 8 and 1115 [Book ref. 23, p. 57].
Chloris striate mosaic virus See GEMINIVIRUSES.
chlorite dismutase See BIOREMEDIATION.
b-chloroalanine A synthetic ANTIBIOTIC which acts e.g. as an
inhibitor of alanine racemase.
chlorobactene See LIGHT-HARVESTING COMPLEX.
Chlorobiaceae A family of non-motile photosynthetic bacteria (suborder CHLOROBIINEAE); species occur e.g. in anaerobic, sulphide-rich freshwater and estuarine muds. The family
includes cocci and rods (some species e.g. Prosthecochloris
aestuarii are prosthecate); GAS VACUOLES occur in Clathrochloris and PELODICTYON. In green-coloured species the predominant
pigments are Bchl c or d and the carotenoid chlorobactene;
in brown-coloured species Bchl e and isorenieratene predominate. The organisms are obligate anaerobic phototrophs; they
are primarily photolithotrophic autotrophs (electron donors: e.g.
sulphur, sulphide thiosulphate in some strains) which fix CO2
by the REDUCTIVE TRICARBOXYLIC ACID CYCLE, but many strains
require vitamin B12 , and all can use simple organic molecules
(e.g. acetate) given a suitable electron donor; elemental sulphur,
when produced, is deposited extracellularly.
Genera: Ancalochloris, CHLOROBIUM (type genus), Clathrochloris, PELODICTYON, Prosthecochloris. (cf. CHLOROHERPETON;
CHLOROPSEUDOMONAS ETHYLICA; CHLOROCHROMATIUM AGGREGATUM.)
[Evidence for bacteria of the Chlorobiaceae in Palaeozoic
seas: Nature (1986) 319 763765.]
Chlorobiineae A suborder of photosynthetic bacteria (order RHODOSPIRILLALES); the organisms contain bacterioCHLOROPHYLL c, d
or e in CHLOROSOMES, and their REACTION CENTRES contain Bchl
a. Families: CHLOROBIACEAE and CHLOROFLEXACEAE. The suborder appears to be taxonomically unsound; thus, on the basis
of RRNA OLIGONUCLEOTIDE CATALOGUING, the species Chlorobium
limicola, C. vibrioforme, Prosthecochloris aestuarii and Chloroherpeton thalassium constitute a moderately tight phylogenetic
group which has no specific relationship with another, somewhat
looser group comprising e.g. Chloroflexus aurantiacus, Herpetosiphon aurantiacus and Thermomicrobium roseum [SAAM
(1985) 6 152156].
Chlorobium A genus of photosynthetic bacteria (family CHLOROBIACEAE). The cells are rods or vibrios, according to species, ca.
12.5 m long; division occurs by binary fission. The genus
includes both green species (C. limicola, C. vibrioforme) and
brown species (C. phaeobacteroides, C. phaeovibrioides).
chlorobium chlorophylls See CHLOROPHYLLS.
chlorobium vesicles Syn. CHLOROSOMES.
Chlorochromatium aggregatum A consortium consisting of an
aggregate of cells: a central, colourless, chemoorganotrophic,
motile bacterium covered by green bacteria of the family
Chlorobiaceae [microanatomy and ecology: JGM (1984) 130
27172723]. Similar consortia, which involve species of the
Chlorobiaceae, are called Chlorochromatium glebulum, Cylindrogloea bacterifera, and Pelochromatium roseo-viride.
Chlorochromatium glebulum See CHLOROCHROMATIUM AGGREGATUM.
Chlorociboria See HELOTIALES.
Chlorococcum
A genus of unicellular green algae (division
CHLOROPHYTA) which differ from CHLORELLA spp e.g. in producing biflagellate zoospores as well as autospores. Species occur
e.g. on damp soil, brick-work, etc.
Chlorophyta
two flagella: a tinsel flagellum directed anteriorly, and a whiplash
flagellum directed posteriorly; a PALMELLOID PHASE commonly
occurs e.g. in Vacuolaria. The numerous yellow-green chloroplasts contain e.g. chlorophylls a and c, b-carotene, and antheraxanthin. Chloromonads occur mainly in freshwater habitats.
chloromycetin Syn. CHLORAMPHENICOL.
Chloromyxum See MYXOSPOREA.
chloroneb (1,4-dichloro-2,5-dimethoxybenzene) An agricultural
systemic ANTIFUNGAL AGENT which is taken up by plant roots
and is concentrated in the roots and lower stem; it is highly
fungistatic for Rhizoctonia spp, moderately fungistatic for
Pythium spp, but shows little activity against Fusarium spp.
It is used as a seed and soil treatment for the control of damping
off etc.
Chloronema A genus of filamentous, mesophilic bacteria (family CHLOROFLEXACEAE [ARM (1981) 35 339364]) which occur
e.g. in lakes. In Chloronema bacterioCHLOROPHYLL d occurs in
chlorosomes.
chloronitrobenzenes (as antifungal agents) These compounds
include several useful agricultural ANTIFUNGAL AGENTS: see e.g.
DICLORAN, QUINTOZENE and TECNAZENE. (See also DINITROPHENOLS.)
chloropeptide (cyclochlorotine) A hepatotoxic MYCOTOXIN produced by Penicillium islandicum (see YELLOW RICE). It appears
to bind to actin within cells, modifying the cytoskeleton.
chlorophenol red Syn. CHLORPHENOL RED.
Chlorophyceae See CHLOROPHYTA.
chlorophycean starch See STARCH.
chlorophylls A class of pigments involved in PHOTOSYNTHESIS;
they may be regarded as derivatives of protoporphyrin IX (see
PORPHYRINS) complexed with magnesium (see figure on page
158). (cf. PHAEOPHYTIN.)
Chlorophylls in algae and cyanobacteria. Chlorophyll a (Chl
a) see figure occurs in all organisms which carry out oxygenic PHOTOSYNTHESIS. Chl b (see figure) occurs in euglenoid
flagellates and green algae (Chlorophyta), as well as in most
higher plants. Chls c1 and c2 occur together in brown algae
(Phaeophyta), chrysophytes, diatoms, and prymnesiophytes,
while Chl c2 without Chl c1 occurs in cryptophytes and dinoflagellates. Chl d occurs in some red algae (Rhodophyta).
Bacteriochlorophylls occur in anoxygenic photosynthetic bacteria (Rhodospirillales). Bchl a is the sole bacteriochlorophyll in most purple bacteria (Rhodospirillineae); those purple
bacteria which lack Bchl a (Ectothiorhodospira abdelmalekii,
E. halochoris, Rhodopseudomonas sulfoviridis, R. viridis, Thiocapsa pfennigii ) have instead Bchl b. Probably all green bacteria
(Chlorobiineae) contain Bchl a usually together with Bchls c
(= chlorobium chlorophyll 660 series) or Bchls d (chlorobium
chlorophyll 650 series). Bchl e is the major bacteriochlorophyll in Chlorobium phaeobacteroides and C. phaeovibrioides,
occurring together with small amounts of Bchl a. Bchl g has
been identified in Heliobacterium chlorum (q.v.). (See also ERYTHROBACTER.)
Chlorophylls generally occur in photosynthetic cells within
specialized membranes or organelles: see CHLOROPLAST, CHLOROSOME, CHROMATOPHORE (sense 2), THYLAKOID. Purified chlorophylls are unstable in the presence of light and oxygen.
Chlorophyta (green algae) A division of the ALGAE, members of
which are characterized by a combination of features: e.g., they
contain chlorophylls a and b, b-carotene, and xanthophylls such
as antheraxanthin, lutein, neoxanthin, violaxanthin and zeaxanthin; the chloroplasts are enveloped by a double membrane but
lack an additional envelope of endoplasmic reticulum; pyrenoids,
Chlorophyta
when present, occur within the chloroplast; the main storage
polymer is starch which is formed within the chloroplast; motile
cells, when formed, bear flagella (commonly 2 or 4) which have
a characteristic structure (see FLAGELLUM (b)).
The green algae (which are not necessarily green in colour)
are a diverse group of organisms which, in vegetative form, may
be unicellular and non-motile (e.g. ANKISTRODESMUS, CHLORELLA,
CHLOROCOCCUM, COCCOMYXA, TREBOUXIA; cf. ACETABULARIA and
DESMIDS), unicellular and flagellated (e.g. CHLAMYDOMONAS,
MICROMONADOPHYCEAE, TETRASELMIS), sarcinoid (e.g. PSEUDOTREBOUXIA), coenobial (e.g. SCENEDESMUS, VOLVOX), filamentous
(e.g. APHANOCHAETE, OEDOGONIUM, SPIROGYRA, STIGEOCLONIUM,
TRENTEPOHLIA, ULOTHRIX; see also SIPHONOCLADOUS), siphonaceous (e.g. CODIUM, DERBESIA, HALIMEDA, OSTREOBIUM), or thallose/parenchymatous (e.g. ENTEROMORPHA, ULVA) reaching a
relatively high degree of structural complexity and differentiation (CHAROPHYTES). Asexual reproduction commonly occurs
by the formation of flagellated zoospores, but some species
may produce e.g. aplanospores (e.g. Aphanochaete, Stigeoclonium), AUTOSPORES, or bulbils (charophytes), or may reproduce by fragmentation of the vegetative thallus (e.g. Spirogyra,
Stichococcus). Sexual reproduction may be isogamous (e.g.
CH2
CH3
C
a
H3C
III
IV
g
10
C
O
CH3
C
phytyl
CH2
CH2
O
N
8
H3C
Mg
CH2CH3
II
OCH3
CHLOROPHYLLS: Chlorophyll a (phytyl = C20 H39 ). Other chlorophylls differ from chlorophyll a as shown below.
Position
Chlorophylls
Chl b
Chl c1
Chl c2
Chl d
Bacteriochlorophylls
Bchl a
Bchl b
Bchls c
Bchls d
Bchls e
Bchl g
Substituent
CHO
CH=CH.COOH
double bond
CH=CH.COOH
double bond
CH=CH2
CHO
3
7
7,8
7
7,8
4
2
CO.CH3
no double bond
phytyl sometimes replaced
by geranylgeraniol
2
CO.CH3
3,4
no double bond
=CH.CH3
4
2
CHOH.CH3
4
C2 H5 , C3 H7 , or C4 H9
5
C2 H5 or CH3
7
phytyl replaced by farnesyl or
stearyl
10
H replaces CO.OCH3
d-methene
CH3
2
CHOH.CH3
4
C2 H5 , C3 H7 , C4 H9 , or
C5 H11
5
C2 H5 or CH3
7
phytyl replaced by farnesyl
10
H replaces CO.OCH3
As for Bchls c, but with CHO at position 3, and phytyl
replaced by farnesyl
3,4
no double bond
=CH.CH3
4
7
phytyl replaced by geranylgeraniol
2
3,4
7
158
chlortetracycline
contains multiple DNA molecules. In at least some higher plants
and algae, ctDNA encodes e.g. the large subunit of RuBisCO,
various subunits of proton ATPase, several cytochromes, and
various rRNAs and ribosomal proteins.
Chloroplast development. The following is a provisional summary. Most chloroplast polypeptides are encoded by nuclear
genes and synthesized on cytoplasmic ribosomes. Such polypeptides are transported into the chloroplast by a post-translational
(rather than co-translational) mechanism. Chloroplast genes,
which may encode up to ca. 100 polypeptides, are essential
for chloroplast development. Chloroplast-encoded polypeptides
and RNAs function within the chloroplast. Light is essential
for chlorophyll synthesis in angiosperms but not in most algae,
mosses, ferns or gymnosperms. [Book ref. 156, pp. 19.]
PROTEIN SYNTHESIS in chloroplasts resembles that in bacteria:
70S-type ribosomes are used, N-formylmethionine is the first
amino acid incorporated, and the process is inhibited e.g. by
chloramphenicol.
Synthesis of galactolipids, the major polar lipids in the
chloroplast, appears to occur in the chloroplast envelope [Book
ref. 156, pp. 193224].
Origin of chloroplasts. Chloroplasts appear to arise either by
the division of existing chloroplasts or by the development of
relatively undifferentiated plastids (proplastids) which lack e.g.
thylakoids and specialized pigments. (See also ETIOPLAST.) The
mechanism of coordination of the expression of nuclear and
chloroplast genes is not fully understood.
[Chloroplasts of giant-celled and coenocytic algae: Bot. Rev.
(1984) 50 267307.]
chloroplast endoplasmic reticulum See CHLOROPLAST.
Chloropseudomonas ethylica A species designation [Book ref.
21] which now appears to refer to a syntrophic mixture of
green sulphide-oxidizing bacteria (Chlorobium limicola and/or
Prosthecochloris aestuarii ) and the sulphur-reducing species
Desulfuromonas acetoxidans.
chloroquine See AMINOQUINOLINES and MALARIA.
Chloros See HYPOCHLORITES.
chlorosis (plant pathol.) The loss of chlorophyll from the tissues
of a plant due e.g. to microbial infection, to the action of
certain phytotoxins, to lack of light, to magnesium or iron
deficiency, etc. Chlorotic tissues commonly appear yellowish
(cf. YELLOWS).
chlorosomes (chlorobium vesicles) Elongated, intracellular, membranous vesicles formed in all members of the CHLOROBIINEAE
grown under appropriate conditions; the vesicles, which contain
most of the light-harvesting (antenna) pigments involved in
PHOTOSYNTHESIS, are attached to, but differ in structure from,
the cytoplasmic membrane. In members of the Chlorobiaceae the
chlorosomes contain bacterioCHLOROPHYLL c, d or e and various
CAROTENOIDS (e.g. chlorobactene in green cells, isorenieratene
in brown cells), while in the Chloroflexaceae they contain
bacteriochlorophyll c and g- and b-carotene; a small amount of
antenna Bchl a is present in the chlorosomes of Chloroflexus
aurantiacus and appears to occur also in the chlorosomes
of members of the Chlorobiaceae. In the Chlorobiineae the
cytoplasmic membrane contains the reaction centre Bchl a together
with a small amount of antenna Bchl a. [Biochemistry of lightharvesting systems: ARB (1983) 52 125157.]
Chlorosplenium See HELOTIALES.
chloroxylenol See PHENOLS.
chlorphenol red A PH INDICATOR: pH 4.86.4 (yellow to red);
pKa 6.0.
chlortetracycline See TETRACYLINES.
Choanephora
bacterial surface (see also BACTERIOPHAGE CTX8). The symptoms of cholera follow secretion and uptake of CHOLERA TOXIN
(q.v.).
Lab. diagnosis. A stool specimen is incubated in alkaline
peptone water for up to 6 hours and the culture used to inoculate
TCBS AGAR. Colonies of interest on TCBS agar should be used to
inoculate (heavily) a non-selective agar medium; growth on this
medium (after 6 hours) may be used for a slide agglutination
test with appropriate antisera. For O139, a rapid screening test
has been developed with monoclonal antibodies [JCM (1998) 36
35953600].
Treatment. Oral or intravenous replacement of fluid and
electrolyte (see e.g. ORAL REHYDRATION SOLUTION). Antibiotics
(e.g. tetracyclines) may help to reduce the period of shedding
and limit the risk of cross-infection (although multidrug-resistant
strains of V. cholerae have been recorded).
Vaccines. A successful live, oral VACCINE against O1 strains
was reported in 1995; however, immunity to O1 does not protect
against O139. Earlier, live vaccines against O139 were being
developed by deletion of certain virulence genes [JID (1994)
170 278283].
(See also NICED; NON-CHOLERA VIBRIOS; NON-VIBRIO CHOLERA.)
cholera toxin (choleragen) A protein ENTEROTOXIN produced by
toxigenic strains of Vibrio cholerae and responsible for the
symptoms of CHOLERA. Cholera toxin (CT) is encoded by genes
ctxA and ctxB of BACTERIOPHAGE CTX8 (toxigenic strains of
V. cholerae are thus lysogenic for this phage).
Structurally, CT resembles PERTUSSIS TOXIN in having the AB5
arrangement of subunits: a pentameric ring of B subunits with
the central A subunit to one side of the plane of the ring. (A
variant of V. cholerae produces B subunits (choleragenoid) but
no A subunits [PNAS (1979) 76 20522056].)
The B subunits bind to glycolipid receptors (GM1 gangliosides) in the brush border membranes of cells lining the small
intestine. Internalization of the toxin occurs via a non-clathrincoated vesicle.
Within the target cell the A subunit is proteolytically cleaved,
but the two fragments remain attached, temporarily, by a
disulphide bond. When the bond is reduced, the active (catalytic)
fragment of the A subunit (responsible for CT activity) acts as
an ADP-ribosyl transferase: it ADP-ribosylates a particular G
protein, Gs , which normally stimulates the activity of ADENYLATE
CYCLASE (AC). As a result, AC is converted to a permanently
active form thus raising the level of cAMP within the target
cell (cf. PERTUSSIS TOXIN). CT activity thus leads to an efflux
of water and electrolyte (sodium and chloride ions) into the
gut lumen, and the profuse watery diarrhoea characteristic of
cholera.
choleragen Syn. CHOLERA TOXIN.
choleragenoid See CHOLERA TOXIN.
cholesterol oxidase An enzyme (EC 1.1.3.6) which oxidizes the
3b-hydroxy group of cholesterol. The enzyme is obtained e.g.
from various actinomycetes (e.g. Nocardia and Streptomyces
spp) and from Schizophyllum commune; it is used in the
detection of cholesterol in body fluids. (See also ENZYMES.)
cholic acid See BILE ACIDS.
choline See e.g. LECITHIN.
chondrioids Syn. MESOSOMES.
chondriosome Syn. MITOCHONDRION.
Chondrococcus (1) A genus of algae of the RHODOPHYTA. (2)
An obsolete bacterial genus; C. columnaris is now Flexibacter
columnaris.
Chondromyces See MYXOBACTERALES.
Chromatium
chondrosarcoma See SARCOMA.
Chondrostereum See APHYLLOPHORALES (Stereaceae).
Chondrus
A genus of marine algae (division RHODOPHYTA).
The thallus consists typically of dichotomously branched fronds
which attach to rocks etc by means of a holdfast. C. crispus
(Irish moss, carragheen moss) is used as a source of
CARRAGEENAN and, in some countries, as food. [Culture of
C. crispus: CJFAS (1986) 43 263268.]
Chonotrichida See HYPOSTOMATIA.
chopped meat medium See COOKED MEAT MEDIUM.
Chorda See PHAEOPHYTA.
Chordaria See PHAEOPHYTA.
Chordopoxvirinae A subfamily of viruses, family POXVIRIDAE,
which infect vertebrates; most members share a common
antigen. Six genera are recognized: AVIPOXVIRUS, CAPRIPOXVIRUS,
LEPORIPOXVIRUS, ORTHOPOXVIRUS, PARAPOXVIRUS, SUIPOXVIRUS.
The members of a given genus are closely related serologically;
genetic recombination can occur between members of a
given genus, and NON-GENETIC REACTIVATION can occur between
members of the same genus and of different genera.
Choreocolax
A genus of algae (division RHODOPHYTA).
C. polysiphoniae is a parasite of another red alga, Polysiphonia
lanosa; the nuclei of C. polysiphoniae apparently enter the
cytoplasm of the host via secondary PIT CONNECTIONS [PNAS
(1984) 81 54205424].
chorioallantoic membrane See EMBRYONATED EGG.
chorismate A central intermediate in the biosynthesis of aromatic
compounds: see Appendix IV(f).
Choristoneura EPVs See ENTOMOPOXVIRINAE.
Christensens urea agar See UREASES.
ChristieAtkinsMunch-Petersen test CAMP TEST.
Chromatiaceae (purple sulphur bacteria; Thiorhodaceae) A
family of photosynthetic bacteria (suborder RHODOSPIRILLINEAE)
which occur typically in sulphide-rich aquatic and terrestrial
habitats (for example, muddy soils, riverine and estuarine
muds); most species contain Bchl a (see CHLOROPHYLLS) the
photosynthetic pigments typically occurring in vesicular
intracytoplasmic membrane systems. The organisms are
primarily photolithotrophic autotrophs which can use e.g.
sulphur, sulphide or hydrogen as electron donors, but at least
some simple organic compounds (e.g. acetate) can be used by all
species under appropriate conditions; sulphur and its compounds
are ultimately oxidized to sulphate, though elemental sulphur can
be deposited intracellularly. Motile species are polarly flagellate
(monotrichous or lophotrichous). GAS VACUOLES occur in some
species. Genera: Amoebobacter, CHROMATIUM (type genus),
LAMPROCYSTIS, THIOCAPSA, Thiocystis, Thiodictyon, Thiopedia,
Thiosarcina, THIOSPIRILLUM; cf. ECTOTHIORHODOSPIRA.
chromatic adaptation In e.g. certain cyanobacteria: adaptation
to changes in the wavelength of incident light by changes in
the composition of the light-harvesting pigments. For example,
Fremyella diplosiphon produces PHYCOBILIPROTEINS allophycocyanin and phycocyanin when grown in red light (ca. 625 nm),
but when grown in green light (ca. 550 nm) the cells also produce phycoerythrin [Book ref. 75, pp. 119126].
chromatid Either of the two longitudinally adjacent threads
formed when a (eukaryotic) CHROMOSOME replicates prior to
MITOSIS; the chromatids are held together at the CENTROMERE.
Sister chromatids are derived from the same chromosome.
ChromaTide See PROBE.
chromatin The fibrous nucleoprotein complex, containing
genomic DNA, HISTONES, NON-HISTONE PROTEINS and RNA,
present in the nucleus of most eukaryotic cells. (The term
chromatography
for example, be stained in situ on the stationary phase e.g.
using specific stains which allow identification of particular types
of molecule.
chromatoid bodies (protozool.) Ribonucleoprotein bodies (commonly rod-shaped) which occur within the young cysts of certain
amoebae (see e.g. ENTAMOEBA). Chromatoid bodies stain well
with iron-haematoxylin (they do not stain with iodine); one, two
or more bodies per cyst may be seen. The nucleoprotein tends
to disperse in the cytoplasm as the cyst ages.
chromatophore (1) One of a number of small membranous vesicles obtained by the experimental disruption of photosynthetic
membranes from bacteria of the Rhodospirillineae; the vesicles are used e.g. for in vitro studies on photophosphorylation.
(2) A system of vesicular, tubular or lamellar membranous structures which occurs in bacteria of the Rhodospirillineae; chromatophores, which contain bacterioCHLOROPHYLL, CAROTENOIDS,
and the electron carriers involved in PHOTOSYNTHESIS, are continuous with the cytoplasmic membrane. (cf. CHLOROSOME.) (3)
Syn. CHLOROPLAST. (4) Syn. CHROMOPLAST.
chromatosome See CHROMATIN.
Chromidina See HYPOSTOMATIA.
Chromobacterium A genus (incertae sedis) of chemoorganotrophic, Gram-negative bacteria which occur e.g. in soil and
water, and as opportunist pathogens in man and other animals.
Cells: round-ended, pigmented (VIOLACEIN-containing) rods, ca.
0.60.9 1.53.5 m, with one polar and one or more lateral
and/or subpolar flagella. Growth occurs on unenriched nutrient
media. Most strains attack glucose fermentatively (forming acid
but usually no gas); some strains attack glucose oxidatively.
Nitrate and nitrite are usually reduced. Growth is inhibited by
6% NaCl. Catalase +ve. Usually oxidase +ve. VP ve. GC%:
ca. 5068. Type species: C. violaceum.
C. fluviatile. Optimum growth temperature ca. 25 C, maximum ca. 30 C. GC%: ca. 5052.
C. lividum. See JANTHINOBACTERIUM.
C. violaceum. Optimum growth temperature ca. 3035 C,
maximum ca. 4044 C. GC%: ca. 6568. (See also MONOBACTAMS and QUORUM SENSING.)
[Book ref. 22, pp. 580582.]
chromoblastomycosis (dermatitis verrucosa; verrucose dermatitis)
A chronic human MYCOSIS, occurring mainly in tropical and
subtropical areas of South America and Africa, caused by any of
several black moulds (e.g. Cladosporium carrionii, Phialophora
spp, Rhinocladiella spp) which are normally saprotrophic e.g. in
soil. Infection occurs via wounds, and warty, spreading, often
ulcerating lesions develop in the skin and underlying tissue.
In the tissues, the fungi occur as thick-walled, dark-brown
muriform cells, 512 m (sclerotic bodies) which multiply by
cell separation (not budding); in culture (e.g. on Sabourauds
dextrose agar) they form slow-growing, velvety, dark-brown to
greenish-black colonies. Pathogenicity may involve the bodys
reaction to fungal components: e.g., lipids extracted from the fungi
can induce granulomatous reactions on intravenous injection into
mice [JGM (1985) 131 187194].
chromogenic Pigment-producing or colour-producing. (cf. ACHROMOGENIC.)
chromomycin (chromomycin A3 ) An ANTIBIOTIC and antitumour
agent containing an aromatic three-ring chromophore linked to
five different sugar residues. Olivomycin and mithramycin are
very similar to chromomycin; all three dyes bind non-covalently
and non-intercalatively to dsDNA, inhibiting synthesis of RNA
and DNA. Binding requires stoichiometric amounts of Mg2+
ions, seems to involve the 2-amino group of guanine, and
Chroomonas
results in a shift in the absorption spectrum of the dye to
longer wavelengths. The dyes are used in cytochemistry as GCspecific fluorochromes, e.g., they produce specific fluorescent
banding patterns in metaphase chromosomes [Science (1977)
195 400402].
chromomycosis May refer either to CHROMOBLASTOMYCOSIS or
to PHAEOHYPHOMYCOSIS.
chromophore That part of a dye molecule which is responsible
for the colour of the dye.
chromoplast (1) A PLASTID in which the main or sole pigments
are CAROTENOIDS. (2) (chromatophore) Any pigmented plastid,
e.g. a CHLOROPLAST or a carotenoid-rich plastid in ripening fruit.
chromosomal fingerprinting See DNA FINGERPRINTING.
chromosome In a prokaryotic cell, or in the nucleus of a
eukaryotic cell: a structure consisting of or containing DNA
which carries genetic information essential to the cell; the
term is also commonly applied to DNA in a mitochondrion or
chloroplast and to the genome of a DNA virus, but generally
not to the genomic RNA of an RNA virus. (cf. GENOME sense 1
and PLASMID.)
(a) Bacterial chromosomes. In most bacteria the chromosome is a ccc dsDNA molecule; in some species (e.g. Borrelia
burgdorferi [Nature (1997) 390 580586], species of Streptomyces) the DNA is linear. Bacterial chromosomes are not
enclosed by a membrane (see PROKARYOTE) but they are apparently linked to the cells cytoplasmic membrane.
Typically, a cell contains only one type of chromosome; the
chromosome may be present in one, several or many copies per
cell depending e.g. on species and on growth conditions; for
example, in Escherichia coli there may be one or more copies
per cell according to the growth rate (see HELMSTETTERCOOPER
MODEL). Some species of bacteria appear normally to have multiple copies of the chromosome e.g. Azotobacter vinelandii may
have an average of 2040 genome equivalents (apparently separate chromosomes) per cell, A. chroococcum contains 2025,
Deinococcus radiodurans has four (in resting cells) to ca. 10,
while Desulfovibrio gigas has ca. 917 (in growing cells) [see
e.g. JGM (1984) 130 15971601, 16031612].
The size of the chromosome (in base-pairs) varies considerably among species. One of the smallest is that of Buchnera,
an obligate intracellular parasite of aphids (640 kb [Nature
(2000) 407 8186]); larger chromosomes occur e.g. in Helicobacter pylori (1.7 106 bp) [Nature (1997) 388 539547]
and Mycobacterium tuberculosis (4.4 106 bp [Nature (1998)
393 537544]).
In Vibrio cholerae the genome consists of two dissimilar
circular chromosomes chromosome 1 (2961 kb) and chromosome 2 (1073 kb) [Nature (2000) 406 477483].
In E. coli the chromosome contains ca. 4.7 106 bp; if
opened out, it would be ca. 1.3 mm in length. Within the cell
it is extensively folded to form a compact structure variously
called a nucleoid, nucleoid body, nuclear area, nucleus etc. The
nucleoid consists mainly of DNA associated with certain types
of protein. The DNA is extensively supercoiled (see DNA), the
degree of supercoiling being determined by the joint activities
of certain enzymes (see TOPOISOMERASE). The supercoiling is
segregated into many topologically distinct domains; a nick in
one domain relaxes the DNA in that domain only. The nucleoid
can be unfolded in vitro by treatment with RNase.
(See also CELL CYCLE and DNA REPLICATION.)
[The chromosome of E. coli : Book ref. 122, pp. 161197,
199227.]
(b) Eukaryotic chromosomes. The eukaryotic NUCLEUS typically contains one or more sets of different chromosomes (see
also PLOIDY; each chromosome is believed to contain a single linear dsDNA molecule complexed with protein (see CHROMATIN).
Between nuclear divisions (interphase) the chromosomes are dispersed as a mass of 30-nm chromatin fibres occupying much
of the volume of the nucleus; during MITOSIS (and MEIOSIS)
each chromosome becomes highly condensed to form a discrete structure with a characteristic morphology (see also KARYOTYPE) and structurally and functionally distinct regions (see e.g.
CENTROMERE and TELOMERE). Chromosome replication (and transcription) occurs during interphase (see CELL CYCLE), so that at
mitosis each chromosome consists of two sister CHROMATIDS.
The 30-nm chromatin fibre in a mitotic chromosome appears
to be organized into a series of loops (each ca. 3090 kb),
the ends of the loops being secured by a central proteinaceous
scaffold ; when the chromosome is treated in vitro to remove
most of the histones and non-histone proteins, the central
scaffold similar in shape to the sister chromatids can be seen
surrounded by a halo of naked DNA loops.
chromosome aberration An abnormality in the number or
structure of chromosomes in a cell. Thus, e.g., a HETEROPLOID
cell may have the diploid number of chromosomes minus
one chromosome (monosomic cell) or plus one chromosome
(trisomic cell). A chromosome may lose a segment (deletion); a
segment may move from one site to another on the same or on
a different chromosome (translocation); a segment may take up
the reverse orientation in the same site (inversion); or a segment
may be duplicated.
chromosome walking A technique with which an unknown
region of a chromosome can be explored. The starting point
is a LIBRARY in which the cloned DNA constitutes a series of
overlapping fragments. A fragment containing a known gene
is selected and used as a probe to identify (e.g. by COLONY
HYBRIDIZATION) other, overlapping fragments which contain the
same gene. The nucleotide sequences of these fragments are
then characterized thus delimiting an overall segment of the
chromosome which comprises the span of the overlapping
sequences. A fragment at one end of this segment is selected,
and the terminal part of this fragment is cleaved and used as a
probe to identify a neighbouring set of overlapping fragments,
and so on.
chromotrope See METACHROMASY.
Chromulina A genus of unicellular CHRYSOPHYTES in which each
cell has a long tinsel flagellum but only a very short second
flagellum. Cysts resemble narrow-necked flasks.
chronic (med.) Refers to a disease which persists for a relatively
long period of time (e.g. months, years) terminating in recovery or death. Examples: LEPROSY; TUBERCULOSIS. (cf. ACUTE.)
chronic bacillary diarrhoea Syn. JOHNES DISEASE.
chronic mucocutaneous candidiasis See CANDIDIASIS.
chronic myelogenous leukaemia See ABL.
chronic wasting disease See TRANSMISSIBLE SPONGIFORM ENCEPHALOPATHIES.
Chroococcales See CYANOBACTERIA.
Chroococcidiopsis
A genus of unicellular CYANOBACTERIA
(section II) in which growth and binary fission lead to the
formation of cubical aggregates of cells; baeocytes are nonmotile and have a fibrous outer cell wall layer at the time of
their release. GC%: 4046.
Chroococcus
A phycological genus of blue-green algae
included in the genus GLOEOCAPSA [JGM (1979) 111 161
(p. 9)].
Chroodactylon See RHODOPHYTA.
Chroomonas See CRYPTOPHYTES.
163
circadian rhythms
cells e.g. ctenophores (comb jellies) and certain cells in the
mammalian respiratory tract.) The structure and ultrastructure
of a cilium are similar to those of the eukaryotic FLAGELLUM
(q.v.); however, cilia are usually shorter (often 710 m) and
they frequently occur in longitudinal rows (see KINETY) or in
specialized groups (see COMPOUND CILIATURE). The characteristic
rhythmical bending of cilia is achieved by the sliding of the
ciliary microtubules relative to one another.
The basic ciliary movement begins with an effective stroke,
i.e., a rapid swing through a wide angle in a straight, relatively
rigid state due to simultaneous activity of the dynein arms
on one side of the axoneme; this is followed by a recovery
stroke in which the cilium returns to its datum position as a
result of the propagation of a wave of dynein activity along
the other side of the axoneme, from base to tip. Energy
is therefore required for both the effective and the recovery
strokes. The rhythmical beating of cilia generates currents in the
ambient fluid thus causing the cell to move or, e.g., propelling
food particles towards the cytostome. (See also METACHRONAL
WAVES.) Many variations of ciliary movement are found among
ciliates including e.g. the ability to change the direction of the
ciliary beating. (See also CLAVATE CILIUM; cf. FLAGELLAR MOTILITY
(b).) [Mechanism and controls of microtubule sliding in cilia:
SEBS (1982) 35 179201; production of different ciliary beat
patterns: SEBS (1982) 35 139157; regulation of ciliary motility
by membrane potential via cAMP in Paramecium: Cell Mot.
(1986) 6 256272.]
(2) (lichenol.) A vegetative appendage which structurally
resembles a RHIZINE but which arises from the margin of a thallus
or apothecium or, in some lichens, from the upper surface of the
thallus.
CIN agar CefsulodinIrgasannovobiocin agar, a medium
developed for the isolation of Yersinia enterocolitica. At least
one strain of Y. enterocolitica (biotype 3B, serotype O3) and
strains of Y. pseudotuberculosis are inhibited on this medium
[JCM (1986) 24 116120].
cin gene See BACTERIOPHAGE P1.
cinchona alkaloids Alkaloids obtained from the bark of certain
tropical trees (especially Cinchona succirubra); the alkaloids
include e.g. cinchonine and QUININE.
cinerubin See ANTHRACYCLINE ANTIBIOTICS.
cingulum See e.g. DIATOMS and DINOFLAGELLATES.
cinoxacin See QUINOLONE ANTIBIOTICS.
CIP Collection de lInstitut Pasteur, Institut Pasteur, 28 Rue du
Docteur Roux, 75724 Paris, Cedex 15, France.
ciprofloxacin See QUINOLONE ANTIBIOTICS.
circadian rhythms In certain parameters of a cell or organism:
rhythmical changes which occur with a periodicity of ca. 24
hours and which may persist for extended periods of time
(e.g. days, weeks) even when the cell or organism has been
isolated from the natural diurnal fluctuations of the environment;
such innate rhythms are often referred to as expressions of a
biological clock.
In eukaryotes, parameters that exhibit circadian rhythms
include e.g. (according to organism): BIOLUMINESCENCE, cell
division, chloroplast ultrastructure, mating type, motility and
photosynthetic activity; thus, for example, peak photosynthetic
activity in Acetabularia occurs with a 24-hour periodicity even
when the organism is kept in continual light. (cf. INFRADIAN
RHYTHMS and ULTRADIAN RHYTHMS.)
Once believed to occur only in eukaryotes, circadian rhythms
have also been detected in some prokaryotes. For example, in the
unicellular cyanobacterium Synechococcus, gene psbAI (which
circannual rhythms
encodes a component of photosystem II) is expressed least at
dawn and maximally at dusk; certain other genes are regulated
in the opposite phase. Under conditions of constant light, the
timing of cell division is influenced by the endogenous 24hour biological clock, even when average doubling time is only
10.5 hours [TIM (1998) 6 407410].
[Molecular bases for circadian clocks (review): Cell (1999) 96
271290. Circadian programmes in cyanobacteria: ARM (1999)
53 389409.]
circannual rhythms In certain parameters of a cell or organism:
rhythmical changes which occur with a periodicity of ca. one
year (see e.g. RED TIDE).
CIRCE See HEAT-SHOCK PROTEINS.
Circinoviridae See TT VIRUS.
circular intensity differential scattering (CIDS) A phenomenon
in which left and right circularly polarized light is scattered in
a characteristic way by a given type of cell, virus, or molecule.
CIDS has been used for the rapid characterization of microorganisms [AEM (1982) 44 10811085].
circularly permuted (mol. biol.) Refers to nucleic acid molecules
in which the bases or genes are arranged in the same sequence
but with different starting points: ABCDEFG, BCDEFGA,
CDEFGAB, etc; such molecules can arise e.g. by cleavage at
different positions in a given type of circular parental molecule.
(See e.g. BACTERIOPHAGE T4.)
circulative transmission (of viruses) (plant pathol.) A mode of
transmission in which viruses taken up by an insect VECTOR pass
from the alimentary canal to the haemolymph and subsequently
to the salivary glands and saliva of the insect; viruses which
are transmitted in this way are called circulative or persistent
viruses. Insects involved in circulative transmission typically
carry plant-infective virions for long periods, sometimes for
life. Circulative transmission characteristically involves a latent
period (several hours to a number of days) during which the
vector, having acquired virus from an infected plant, is unable
to transmit the virus to a healthy plant. (cf. NON-CIRCULATIVE
TRANSMISSION.)
Some viruses (e.g. potato yellow dwarf virus, wound tumour
virus) replicate in their insect vectors; circulative transmission
of such propagative viruses is termed propagative transmission.
Other viruses (e.g. barley yellow dwarf virus) apparently do
not replicate in their insect vectors; circulative transmission of
such non-propagative viruses is accordingly referred to as nonpropagative transmission.
circulative viruses See CIRCULATIVE TRANSMISSION.
circulins See POLYMYXINS.
circumsporozoite protein See PLASMODIUM.
cirramycin See MACROLIDE ANTIBIOTICS.
cirri See CIRRUS.
cirrus (pl. cirri) A discrete group of somatic cilia (several to
over 100) which act primarily as a unified locomotive organelle;
the typical cirrus is conical. Cirri are characteristic of the
HYPOTRICHIDA. (See also COMPOUND CILIATURE.)
cis-acting See CIS-DOMINANCE.
cis-dominance The phenomenon in which a genetic element (a
gene or a non-coding sequence such as a promoter) affects only
the DNA molecule in which it occurs; in a COMPLEMENTATION
TEST, a mutant form of such a genetic element (which is called a
cis-acting element) cannot be complemented by (i.e., is dominant
over) the wild-type form of the element present in the same cell.
The converse of a cis-acting element is a trans-acting element,
an element which encodes a product that can diffuse through
the cytoplasm and act on other DNA molecules. For example,
Cladosporium
C. freundii. Indole ve; malonate (usually) ve; H2 S + ve;
growth in KCN media. Nitrogen fixation has been reported in
some strains. Serotypes may be distinguished on the basis of
O and H antigens, some of which are common to serotypes
of Escherichia and Salmonella; C. freundii H antigens are
monophasic. Certain strains are reported to have a Vi antigen
serologically identical to that of Salmonella typhi (see VI
ANTIGEN), but its presence is not related to virulence. (See also
PHASE VARIATION.)
Citrobacter spp may be isolated from human or animal faeces,
from various clinical specimens, and from food, water, sewage,
soil etc; they may be opportunist pathogens. C. freundii and
C. diversus have been associated with cases of human diarrhoea.
[Book refs. 22, pp. 458461, and 46, pp. 11401147.]
citrovorum factor See FOLIC ACID.
L-citrulline See e.g. Appendix IV (a).
Citrus exocortis viroid See VIROID.
Citrus leaf rugose virus See ILARVIRUSES.
Citrus leprosis virus See RHABDOVIRIDAE.
Citrus tristeza virus A member of the CLOSTEROVIRUSES which
causes tristeza disease of citrus trees; the virus has killed
millions of orange trees in Brazil.
Citrus variegation virus See ILARVIRUSES.
CJD CREUTZFELDTJAKOB DISEASE.
CL region See IMMUNOGLOBULINS.
Cladobotryum See HYPHOMYCETES and HYPOMYCES.
cladogram Any dendrogram which expresses phylogenetic relationships. (cf. PHENOGRAM.)
Cladonia
A large genus of LICHENS (order LECANORALES);
photobiont: a green alga. Species tend to be variable in
appearance. There is a granular or squamulose primary thallus (often evanescent, but predominant in some species) from
which may arise hollow podetia (see PODETIUM); according to
species, podetia may be awl-shaped, branched and shrubby, or
funnel-, cup- or wine-glass-shaped, and may bear brown or
red hymenial discs (apothecia). Species occur on the ground
(particularly on peaty soils in heaths and moors), on walls,
on decaying logs, etc. Some species e.g. C. portentosa (formerly C. impexa), C. rangiferina, C. stellaris form cushions
of extensively branched podetia (reindeer moss) on the ground
in mountainous regions of Europe and in Arctic regions, where
they may serve as an important source of winter fodder for reindeer and caribou.
Cladophora A genus of filamentous, branched, siphonocladous
green algae (division CHLOROPHYTA); the filaments are composed
of cylindrical, multinucleate cells, the walls of which contain
parallel arrays of cellulose microfibrils. An isomorphic alternation of generations occurs; sporophytes produce quadriflagellate, uninucleate zoospores, gametophytes produce biflagellate
isogametes. Species occur in freshwater and marine habitats,
sometimes free-floating, but usually attached to a substratum by
rhizoids; some species often form extensive tangled skeins up
to several metres in length (blanket weed).
Cladosiphon See PHAEOPHYTA.
cladosporiosis Any human or animal disease caused by a species
of CLADOSPORIUM.
Cladosporium
A genus of fungi (class HYPHOMYCETES)
which form septate mycelium and dark-coloured, aseptate or
septate, ellipsoidal conidia. The organisms include saprotrophs
and pathogens of plants and animals. Species include e.g.
C. carrionii (see e.g. CHROMOBLASTOMYCOSIS), C. cucumerinum
(see e.g. GUMMOSIS), C. herbarum (teleomorph: Mycosphaerella
tassiana) (see e.g. BLACK SPOT (sense 1), SAP-STAIN, TEXTILE
Citeromyces
A genus of yeasts (family SACCHAROMYCETACEAE). Cells reproduce by multilateral budding; neither
pseudomycelium nor true mycelium is formed. Asci are
persistent and contain one (occasionally two) rough-surfaced
spheroidal spores. Glucose is fermented; NO3 is assimilated.
One species: C. matritensis (anamorph: Candida globosa),
isolated from e.g. fruit preserved in syrup, tree exudates etc.
[Book ref. 100, pp. 117119.]
Citifluor A photofading retardant and mountant used e.g. for
epifluorescence microscopy of soil [SBB (1985) 17 739746].
citrate metabolism See e.g. TCA CYCLE, CIT PLASMID, DIACETYL;
see also CITRIC ACID.
citrate synthase See Appendix II(a).
citrate test An IMVIC TEST which determines the ability of a
bacterial strain to use citrate as the sole source of carbon (see
e.g. TCA CYCLE). A saline suspension of the test organism is
prepared from growth on a solid medium. An inoculum from
this suspension is transferred by means of a STRAIGHT WIRE to the
test medium (e.g. KOSERS CITRATE MEDIUM or SIMMONS CITRATE
AGAR); the wire is dipped (ca. 1 cm) into the suspension and
then dipped into, or streaked across, the test medium. Such a
small inoculum minimizes carry-over of nutrients and avoids
causing turbidity in Kosers medium. The inoculated medium is
incubated and examined daily for evidence of growth (turbidity
in Kosers medium, blue coloration in Simmons medium);
growth is a positive reaction.
citreoviridin A yellow pigment and neurotoxic MYCOTOXIN produced by Penicillium citreoviride growing e.g. on polished rice.
(See also YELLOW RICE.) The molecule consists of a hydrofuran ring linked, via a conjugated polyene, to an a-pyrone
chromophore; it emits a brilliant yellow fluorescence on UV
irradiation. Consumption, by man, of rice contaminated with citreoviridin may be responsible for acute cardiac beriberi : a fatal
disease characterized by ascending paralysis, convulsions, and
respiratory arrest; these symptoms can be reproduced in animals
by feeding them with citreoviridin. In vitro, citreoviridin inhibits
PROTON ATPASE isolated e.g. from mitochondrial membranes.
citric acid A tricarboxylic acid present e.g. in many fruits
(especially citrus fruits) and an important metabolic intermediate
in many organisms (see e.g. TCA CYCLE). Citric acid is obtained
commercially mainly from strains of Aspergillus niger grown
e.g. on molasses or starch hydrolysates; the accumulation of
citric acid is apparently due to abnormal functioning of the TCA
cycle. The citric acid is separated from the fermentation liquor by
precipitation as the Ca2+ salt. Citric acid has many commercial
uses e.g. as an acidifying agent in various foods, beverages
and pharmaceuticals. [Production methods etc: Book ref. 8, pp.
709747.]
citric acid cycle Syn. TCA CYCLE.
citrinin A yellow pigment and MYCOTOXIN produced by Penicillium spp in mouldy cereals etc. It is nephrotoxic e.g. in pigs.
Citrobacter A genus of Gram-negative bacteria of the ENTEROBACTERIACEAE (q.v.). Cells: ca. 1 26 m, usually motile. MR
+ve; VP ve citrate +ve; acid and gas from glucose; lactose
+ve or ve, or fermented slowly. Growth usually occurs on/in
selective media such as DCA, SS agar, tetrathionate broth and
selenite broth. GC%: 5052. Type species: C. freundii.
C. amalonaticus (formerly e.g. C. intermedius biotype a;
Levinea amalonatica). Indole +ve; malonate ve; H2 S ve;
growth in KCN media.
C. diversus (= C. koseri ; formerly e.g. C. intermedius biotype b; Levinea malonatica). Indole +ve, malonate +ve and
H2 S ve; no growth in KCN media.
167
Cladostephus
clavems A class of antibiotics; a clavem contains a clavam-like
nucleus in which a double bond occurs between C-2 and C-3
(see b-LACTAM ANTIBIOTICS, Figure (f)).
Clavibacter A genus of Gram-positive, asporogenous, non-acidfast, non-motile, obligately aerobic, phytopathogenic coryneform
bacteria; C. xyli subsp. xyli causes ratoon stunting disease
of sugarcane, C. xyli subsp. cynodontis causes Bermuda-grass
stunting disease. [IJSB (1984) 34 107117.]
Claviceps A genus of fungi (order CLAVICIPITALES) which are
typically parasitic on grasses (see e.g. ERGOT; see also PASPALUM
STAGGERS).
C. purpurea. The cycle of infection begins when ascospores
germinate and infect the ovaries of a susceptible grass. The
fungus soon produces small, colourless conidia (the Sphacelia
stage) which become suspended in a HONEYDEW secretion
(possibly produced by the plant in response to infection);
insects, attracted by the honeydew, disperse the conidia to the
ovaries of uninfected grasses. Later, the fungus produces a
SCLEROTIUM (q.v.) (the ergot, the overwintering stage) in the
position normally occupied by the grain. In spring or early
summer the sclerotia germinate, each giving rise to several erect,
drum-stick-like stromata; perithecia develop in the surface layer
of each stromal head, their ostiolar pores level with the stromal
surface. Each ascus contains 8 thread-like ascospores.
Clavicipitales An order of fungi (subdivision ASCOMYCOTINA)
which include entomogenous species, and species parasitic on
other fungi or on grasses. Ascocarp: perithecioid, superficial or
immersed in a stroma. Asci: unitunicate, cylindrical, with a thick
apical cap. Ascospores: elongated to filiform, often multiseptate,
sometimes fragmenting. Genera: e.g. Acrospermum, Balansia,
CLAVICEPS, CORDYCEPS, EPICHLOE , Hypocrella, HYPOMYCES.
claviformin Syn. PATULIN.
clavine alkaloids See ERGOT ALKALOIDS.
Clavispora A genus of yeasts (family SACCHAROMYCETACEAE)
which reproduce by multilateral budding; pseudomycelium may
be formed. Asci are formed following conjugation between
cells of different mating type. Ascospores: clavate, minutely
warty, 14 per ascus. Glucose is fermented; NO3 is not
assimilated. One species: C. lusitaniae (anamorph: Candida
lusitaniae), isolated e.g. from pigs and from human skin and
sputum. [Book ref. 100, pp. 120122.]
clavulanic acid A clavam (see b-LACTAM ANTIBIOTICS for
structure). Clavulanic acid, produced e.g. by Streptomyces
clavuligerus (ATCC 27064), binds to the PENICILLIN-BINDING
PROTEINS of Escherichia coli (preferentially to PBP-2) but
has only weak antibacterial activity; however, it is a potent
inhibitor of many b-LACTAMASES from Gram-positive and
Gram-negative bacteria and may thus be used in combination
with b-lactamase-sensitive antibiotics (see e.g. AUGMENTIN and
TIMENTIN). Clavulanic acid is unstable as the free acid and is
isolated from aqueous solutions as a salt.
CLB (coccidian-like body) An organism linked with prolonged
diarrhoea (duration: weeks) in humans; it appears to be waterborne. [Epidemiology: Lancet (1993) 341 11751179.]
cleared lysate The supernatant obtained when bacteria in suspension are lysed and centrifuged for ca. 1020 min at ca. 20000 g;
it may contain plasmids (if present in the cells) but is generally
free of particulate cell debris and chromosomal DNA.
clearing In preparing a specimen for microscopy: the stage in
which the dehydrating agent (usually ethanol) is replaced by a
solvent (clearing agent ) such as benzene, xylene, or terpineol;
if the cleared specimen is to be mounted in a MOUNTANT or
impregnated with paraffin wax, the clearing agent must be
168
cloning
or for synthesis of the product encoded by the sequence (see
EXPRESSION VECTOR).
Initially, the required gene (or other sequence) is inserted
(spliced) into a REPLICON often a PLASMID or a phage genome.
The replicon functions as a vector (= cloning vector ), i.e. a
molecule which, on being replicated in a cell, brings about the
replication of the given gene (as the latter is an integral part of
the vector).
The insertion of a gene into a plasmid vector is carried out in
a procedure involving a RESTRICTION ENDONUCLEASE and a ligase
(see figure).
Vector molecules, each incorporating the given gene, are introduced into cells in which they can replicate; plasmid vectors are
introduced into bacteria by TRANSFORMATION or ELECTROPORATION. The cells, containing vectors, are then cultured; because
a bacterial population can reach very high numbers in culture,
and because each cell contains one or more copies of the vector,
large numbers of vector molecules (each containing the given
gene) are obtained i.e. the gene has been cloned.
To harvest the cloned gene, the cells are lysed and the
vector molecules are isolated e.g. by isopycnic centrifugation
(cf. QIAGEN PLASMID KIT). The cloned gene is then cut from each
vector molecule (by means of the original restriction enzyme),
and copies of the cloned gene are separated from vector DNA
e.g. by gel electrophoresis.
Cloning with plasmid vectors in bacteria.
During the initial stage (see figure), one potential problem
is that some plasmid molecules may re-circularize without
incorporating a copy of the gene; such plasmids may then be
taken up by transformation but, lacking the gene insert, they
would not contribute to the cloning process. This difficulty may
be addressed by pre-treating the cleaved (linearized) plasmids
with a phosphatase to remove the 5 -phosphate groups which
are necessary for ligase action and re-circularization. When the
gene (target) fragments are added, their 5 -phosphate groups can
be ligated to 3 -OH ends in the plasmids, resulting in stable,
circular hydrid plasmids which contain single-stranded nicks (at
the 5 -OH ends). These hybrid plasmids can then be used for
transformation the nick sites being repaired in vivo to yield
ccc dsDNA molecules.
Sometimes the target fragment lacks restriction sites, or
has incompatible ones. This problem may be addressed as
follows. Sticky ends, if present, are changed to blunt ends (see
BLUNT-ENDED DNA); this may be achieved by either removing
single-stranded overhangs (e.g with ENDONUCLEASE S1) or by
synthesizing a complementary strand on each 5 overhang
(thus converting 5 overhangs to dsDNA). To each blunt end
can now be ligated a short, blunt-ended dsDNA molecule a
linker which contains a suitable restriction site; one example
of a linker is:
5 -GGAATTCC-3
3 -CCTTAAGG-5
which contains the EcoRI restriction site (see table in RESTRICBecause a linker is a PALINDROMIC
sequence is the same in both strands)
either end can be ligated. Blunted-ended ligation requires a
higher concentration of enzyme, a lower temperature and a
longer time. (See also ADAPTOR.)
Following transformation, only cells which have actually
received a plasmid can contribute to the cloning process. These
cells can be selected for if the plasmid vector contains an
antibiotic-resistance gene; thus, if the transformed cells are
TION ENDONUCLEASE).
SEQUENCE (the 5 -to-3
169
GA
AT
(a)
plasmid
C T T A
T
GA A T
AA
TT
CT
TC
AA
TT
A
TA
'foreign' DNA
restriction
endonuclease
Eco RI
restriction
endonuclease
Eco RI
G
T
CT
A AT T C
(b)
A AT
AA
TC
G
C
TT
G AA
AA
C T T
CT TAA
(c)
G A AT T
C TTA A
ligase
(d)
hybrid plasmid
CLONING: insertion of a gene (or other foreign DNA) into a plasmid vector (diagrammatic).
(a) A plasmid and a piece of foreign DNA. Both molecules contain the nucleotide sequence GAATTC which is recognized by the RESTRICTION
ENDONUCLEASE EcoRI; in the foreign DNA, the sequence to be cloned lies between the two restriction sites. EcoRI cuts between the guanosine
(G) and adenosine (A) nucleotides, as shown by the arrows.
(b) As a result of EcoRI activity, the plasmid has been linearized, and both types of molecule now have sticky ends, i.e. terminal,
single-stranded complementary sequences of nucleotides (5 -AATT).
(c) The foreign DNA has integrated with the plasmid vector molecule through base-pairing between complementary nucleotides in the sticky
ends.
(d) An enzyme, DNA ligase, has catalysed a phosphodiester bond between the sugar residues of each G and A nucleotide, forming a
hybrid plasmid (recombinant plasmid; also referred to as hybrid DNA, or hDNA). Note that, unless prevented, at least some of the vector
molecules may simply re-circularize by base-pairing between their sticky ends; such re-circularization, which would reduce the efficiency of
the procedure, may be prevented by treating the linearized plasmids with phosphatase (see entry).
A population of hybrid plasmids can be inserted into bacteria by transformation or electroporation for cloning. Note that, if required, the
(cloned) fragment can be cut from the vector by using the same restriction enzyme.
Reproduced from Bacteria 5th edition, Figure 8.6, page 182, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
170
Clostridium
plated on a medium containing the relevant antibiotic, only the
plasmid-containing cells (which are resistant to the antibiotic)
will form colonies.
Some vectors are particularly useful in that, following transformation, they can signal the uptake of both vector and
DNA insert. For example, in plasmid pBR322 (see PBR322), the
tetracycline-resistance gene contains a BamHI restriction site,
and the ampicillin-resistance gene contains a PstI restriction site;
if, for example, PstI is used to insert the gene (analogous to
EcoRI in the figure), then any transformant which is (i) sensitive
to ampicillin but (ii) resistant to tetracycline may be presumed
to contain the complete hybrid plasmid.
A different approach to selection is provided by REPRESSOR
TITRATION.
If a plasmid vector replicates under relaxed control (see
PLASMID), the number of plasmids per cell can be greatly
increased by treating the cells with chloramphenicol; in this way,
the yield of cloned product can be maximized.
Cloning with phage vectors in bacteria.
In some phages (e.g. BACTERIOPHAGE LAMBDA) the genome
contains a fairly high proportion of non-essential DNA; thus,
a sequence may be excised from the genome, using restriction
endonucleases, and replaced by the fragment to be cloned. Such
a vector is called a REPLACEMENT VECTOR; using the genome of
phage lambda as a replacement vector it is possible to clone
a fragment of about 20 kb (compared with <10 kb in plasmid
pBR322). Even larger fragments, up to 40 kb, can be cloned
in a COSMID.
Phage genomes can be used as vectors only if the recombinant
genome (i.e. genome plus insert or fragment) is not too large to
fit into the phage head, and only if it contains, where necessary,
the appropriate packaging signals.
Once incorporated into a phage particle, the recombinant
genome can be injected into bacterial cells and will replicate like
a plasmid. (Note that, during construction of a phage vector, any
sequences in the phage genome that promote integration into the
bacterial chromosome should be removed.)
ssDNA phages may also be used as vectors; filamentous
phages have the advantage that their virions can accomodate
a wide range of sizes of target DNA. Another option for cloning
is a hybrid vector which includes sequences from a phage and
a plasmid: see PHAGEMID.
Characterization of clones.
Sometimes, clones are prepared from a mixture of DNA fragments or from a LIBRARY, i.e. different cells within the culture
will contain vectors that incorporate different fragments of DNA.
In such cases one can screen for cells that contain a particular
gene or sequence. Screening methods include: COMPLEMENTATION
analysis (in which cells are selected when their particular fragment of cloned DNA complements a given chromosomal defect);
probing for a specific gene product (e.g. by using labelled antibodies); or hybridization techniques (see e.g. COLONY HYDRIDIZATION).
Linguistic note.
The above account of cloning should make it clear that a gene
(or other sequence) is inserted into a vector, and that a vector
(and its insert) is cloned in a population of cells. Unfortunately,
the expression cloned into.. . . has become widely used in
the literature; this piece of gibberish has been promulgated by
mindless repetition. A given sequence of DNA may be cloned
in a particular vector molecule or cloned in a particular type of
cell.
Clonothrix A genus of IRON BACTERIA which occur as sheathed,
tapering filaments. Type species: C. fusca.
Clostridium
energy by the STICKLAND REACTION, and in some species this
is the preferred mode of energy metabolism. Certain species
(e.g. C. perfringens, C. sordellii ) are both proteolytic and saccharolytic, while others are restricted to specific substrates (see
e.g. C. cochlearium, C. cylindrosporum and C. kluyveri ). Some
species can reduce nitrate. Some clostridia are thermophilic, others are psychrophilic, but most are mesophilic. GC% range for
the genus: ca. 2255. Type species: C. butyricum.
Currently, >80 species (some listed below) but see end of
entry.
C. aceticum. Saccharolytic; diazotrophic; acetic acid is formed
from CO2 and H2 . (See also ANAEROBIC DIGESTION.)
C. acetobutylicum. Proteolytic and saccharolytic; growth
requirements appear to include PABA and biotin. (See also
ACETONEBUTANOL FERMENTATION.)
C. acidiurici. A species metabolically similar to C. cylindrosporum (q.v.)
C. barati. Incorporates the former species C. perenne and
C. paraperfringens [IJSB (1982) 32 7781]. (See also BOTULINUM TOXIN.) LIPASE ve, LECITHINASE +ve.
C. barkeri. Saccharolytic; butyric and lactic acids, CO2 and
H2 are formed from carbohydrates.
C. beijerinckii. Saccharolytic: butyric and acetic acids and
butanol are formed from glucose.
C. bifermentans. Proteolytic and saccharolytic; requires e.g.
biotin, nicotinamide, pantothenate, pyridoxine and various amino
acids. Spores: ovoid, subterminal. Indole-positive. The organisms form a lecithinase similar to the a-toxin of C. perfringens.
C. botulinum. The causal agent of BOTULISM (see also
BOTULINUM TOXIN). Cells: motile, ca. 0.31.9 3.49.4 m;
spores: ovoid, subterminal. All strains can ferment glucose (none
can use lactose, mannitol or sucrose), and all form metabolic
products which include acetic and butyric acids. All strains can
hydrolyse gelatin and produce lipases. The organisms are divided
into seven types (designated A, B, C, D, E, F and G), strains of a
given type producing a BOTULINUM TOXIN which is antigenically
distinct from those of the other types; in some cases the strains of
a given type are metabolically heterogeneous: e.g., type B strains
include some which are saccharolytic as well as some which are
both proteolytic and saccharolytic. Minimum growth temperatures: often ca. 10 C, but ca. 3.3 in saccharolytic type B strains
and in type E strains. Minimum pH for growth is sometimes
reported to be ca. 4.6 for types A and B, and ca. 5.0 for type E;
under certain conditions growth and toxin formation may occur
at pH values down to ca. 4.0 [Nature (1979) 281 398399]. The
heat-resistance of endospores is strain-dependent; thus, e.g., for
types A and B the D112.8 (see D VALUE) is ca. 0.151.32 min,
for type C the D100 is ca. 0.12 min (terrestrial strains) or ca.
0.40.9 min (marine strains), and for type E the D80 is ca.
0.333.3 min (in media) or ca. 1.64.3 min (in fish) [Book
ref. 30, p. 327].
C. botulinum type A strains are proteolytic and saccharolytic;
they cause botulism in man and other animals (see also
LIMBERNECK).
C. botulinum type B strains are either saccharolytic or proteolytic and saccharolytic; they cause botulism in man and other
animals.
C. botulinum type C strains are proteolytic and saccharolytic;
they cause botulism in animals: see e.g. FORAGE POISONING,
MIDLAND CATTLE DISEASE, WESTERN DUCK DISEASE.
C. botulinum type D strains are proteolytic and saccharolytic;
they cause botulism in animals (see LAMZIEKTE).
C. botulinum type E strains are saccharolytic; they are often
associated with fish and fish products, and they cause botulism
Clostridium
C. propionicum. See PROPIONIC ACID FERMENTATION.
C. ramosum (formerly e.g. Ramibacterium ramosum). Saccharolytic; ferments glucose, maltose, lactose, sucrose and
salicin, forming acetic acid as a main product. Cells frequently
stain Gram-negatively and are non-motile; spores: spherical to
ovoid, terminal, but seldom observed.
C. septicum. Proteolytic and saccharolytic; glucose, maltose,
lactose and salicin are fermented with the formation of acetic and
butyric acids, and gelatin is hydrolysed. Spores: ovoid, subterminal. Toxins formed: a-toxin (dermonecrotizing, haemolytic),
b-toxin (a DNase), g-toxin (a hyaluronidase) and d-toxin (a
THIOL-ACTIVATED CYTOLYSIN). A causal agent in GAS GANGRENE
and in BRAXY and MALIGNANT OEDEMA. (See also NEUTROPENIC
ENTEROCOLITIS.)
C. sordellii. Proteolytic and saccharolytic; glucose and maltose are fermented to e.g. acetic acid. Gelatin is hydrolysed,
and milk is digested. Indole-positive. Urease-positive. Some
strains form a lecithinase (a-toxin) and e.g. a THIOL-ACTIVATED
CYTOLYSIN. [Taxonomy of lecithinase-negative strains: JGM
(1985) 131 16971703.] Spores: ovoid, subterminal. (See also
MALIGNANT OEDEMA.)
C. sphenoides. Saccharolytic; glucose, maltose, salicin and
mannitol are fermented to e.g. acetic acid. Reported to be capable
of growth on citrate. Some strains hydrolyse gelatin and some
produce indole. Cells typically stain Gram-negatively. Spores:
spherical, subterminal to terminal.
C. spiroforme. Saccharolytic; carbohydrates are fermented to
acetic (not butyric) acid. Cells: helical.
C. sporogenes. Proteolytic and saccharolytic; glucose and
maltose are fermented to e.g. acetic and butyric acids. Gelatin
is hydrolysed, and milk is digested. Spores: ovoid, subterminal.
C. subterminale. Proteolytic; gelatin is hydrolysed, and milk
is digested. Lysine is fermented to e.g. acetic and butyric acids.
Spores: ovoid, subterminal.
C. tertium. Saccharolytic; glucose, maltose, lactose, sucrose,
salicin and mannitol are fermented to acetic and butyric
acids. Spores: ovoid, terminal. Growth occurs aerobically on
blood agar.
C. tetani. The causal agent of TETANUS. (See also TETANOSPASMIN and THIOL-ACTIVATED CYTOLYSIN.) Proteolytic; gelatin is
hydrolysed, and acetic and butyric acids are formed from the
fermentation of peptones. No carbohydrates not even glucose are fermented. Some strains form indole. Spores: spherical and terminal.
C. thermoaceticum. See ACETOGENESIS.
C. thermocellum. Saccharolytic; cellobiose, CELLULOSE and
hemicellulosic materials are degraded and fermented, the main
products being ethanol, acetic acid, CO2 , and H2 . (See also CELLULASES and CELLULOSOME.) [Regulation of cellulase formation:
JGM (1985) 131 23032308.] Pentoses are apparently not utilized. Optimum growth temperature: 5560 C.
C. thermolacticum. Saccharolytic; thermophilic. A wide range
of carbohydrates (including xylan) can be fermented, the main
product being L(+)lactate. Some strains are cellulolytic. [SAAM
(1985) 6 196202.]
C. thermosaccharolyticum. Saccharolytic; many carbohydrates
(including e.g. GLYCOGEN, PECTINS and STARCH) are fermented to
e.g. acetic, butyric and lactic acids, CO2 , and H2 . Optimum
growth temperature: 5560 C. Spores may have a D VALUE of
ca. D120 = 4 min; the organisms are sometimes responsible for
hard SWELL spoilage of canned foods. (See also CANNING.)
C. thermosulfurogenes. Saccharolytic. Cells are peritrichous,
Gram ve; filaments may occur. Spores: spherical. Opt. growth
clostripain
at >60 C. In microbial mats from hot volcanic springs. [JGM
(1983) 129 1149.]
C. villosum. Isolated from subcutaneous abscesses in cats
[IJSB (1979) 29 241244].
C. welchii. See C. perfringens.
Other species include e.g. C. aurantibutyricum, C. celatum,
C. cellobioparum, C. coccoides, C. durum, C. fallax, C. felsineum, C. formicoaceticum, C. glycolicum, C. haemolyticum,
C. indolis, C. lituseburense, C. oceanicum, C. putrefaciens,
C. putrificum, and C. sticklandii.
The genus Clostridium is heterogeneous, and proposals for rationalization have included the creation of a number of new genera
(Caloramator, Filifactor, Moorella, Oxobacter and Oxalophagus)
[IJSB (1994) 44 812826].
clostripain A thiol PROTEASE (MWt ca. 50000; EC 3.4.22.8),
obtained from Clostridium histolyticum, which acts specifically
at basic amino acyl (arginyl, lysyl) residues. It also has amidase
and esterase activity, cleaving amides and esters of amino acids.
clot culture BLOOD CULTURE in which clotted blood, minus serum,
is liquefied (e.g. with STREPTOKINASE) and the resulting fluid used
as the inoculum. Apparently not widely used due e.g. to the
risk of contamination prior to the inoculation stage.
clotrimazole (bis-phenyl-(2-chlorophenyl)-1-imidazole methane)
One of the earliest of the clinically useful imidazole antifungal
agents (see AZOLE ANTIFUNGAL AGENTS); it is used topically in
the treatment of superficial mycoses (e.g. candidiasis, ringworm,
pityriasis versicolor).
clotting (of blood plasma) See FIBRIN; COAGULASE; ANTICOAGULANT.
clover blackpatch disease See SLAFRAMINE.
clover rot (clover sickness; sclerotinia crown and stem rot, SCSR)
A disease of clover and other forage legumes caused by Sclerotinia spp (particularly S. trifoliorum). Leaves and petioles of
infected plants turn olive-brown and subsequently rot; the disease
progresses from the petioles to the stem and root, leading to the
death of the plant. Control by repeated applications of e.g. benomyl or quintozene is effective but economically impracticable.
[Review: Bot. Rev. (1984) 50 491504.]
clover wound tumour virus Syn. WOUND TUMOUR VIRUS.
clover yellow mosaic virus See POTEXVIRUSES.
clover yellows virus See CLOSTEROVIRUSES.
cloverleaf structure (of tRNA) See TRNA.
cloxacillin See PENICILLINS.
club fungi See APHYLLOPHORALES (Clavariaceae).
clubroot A disease of cruciferous plants (cabbages, cauliflowers,
turnips etc) caused by Plasmodiophora brassicae (see PLASMODIOPHOROMYCETES). The roots of an infected plant become swollen
and distorted, developing a single large gall (the club symptom) or clusters of smaller galls (finger-and-toe disease). The
aerial parts of the plant may be stunted and may wilt in hot
weather; the foliage often acquires a reddish tinge. Secondary
infection of the galls by SOFT ROT bacteria commonly occurs.
P. brassicae causes both hyperplasia and hypertrophy of
infected tissues, apparently by inducing hyperauxiny (see
AUXINS). Healthy plant tissue normally contains, in separate
compartments, an indole compound, glucobrassicin, and an
enzyme (glucosinolase) which hydrolyses glucobrassicin to
indoleacetonitrile (IAN), a precursor of indoleacetic acid (IAA).
P. brassicae apparently interferes with the compartmentalization
of glucobrassicin and glucosinolase, resulting in increased levels
of IAN (and hence IAA) in infected tissues.
The cysts of P. brassicae can remain viable for years in the
soil, and it is difficult to eradicate the disease from contaminated
cobweb disease
tract and/or various other tissues; they may be mild to fatal.
Coccidioses of domestic animals and poultry are often of
economic importance.
(a) Poultry. In chickens, Eimeria necatrix causes severe haemorrhage in the small intestine, and E. tenella causes haemorrhage and necrosis in the caecum; other pathogens include
e.g. E. acervulina and E. brunetti. In ducks, Tyzzeria perniciosa
causes haemorrhagic intestinal disease. In turkeys, severe inflammation of the intestine is caused by e.g. E. adenoeides and
E. meleagrimitis.
(b) Domestic animals. In cattle, haemorrhagic lesions in the
intestine are caused e.g. by E. bovis and E. zurnii (E. zuernii );
an increased incidence of disease may occur during cold
weather (winter coccidiosis). In sheep, intestinal disease may
be caused e.g. by E. ahsata, E. ovina or E. ovinoidalis. In
pigs, enteritis, severe diarrhoea and emaciation are caused
e.g. by E. scabra. In rabbits, intestinal disease (often fatal) is
caused e.g. by E. magna and E. irresidua; E. stiedae (E. stiedai)
causes diarrhoea, enlargement of the liver and bile ducts, and
emaciation. In cats, intestinal symptoms may be due to infection
by Isospora spp (which may also infect dogs) or Toxoplasma
(see TOXOPLASMOSIS). (cf. SARCOSPORIDIOSIS; see also EQUINE
PROTOZOAL MYELOENCEPHALITIS.)
(c) Man. Infections involving Isospora belli and I. hominis are
believed to be commonly asymptomatic, but intestinal symptoms
may occur. (See also CRYPTOSPORIDIOSIS, SARCOSPORIDIOSIS and
TOXOPLASMOSIS.)
Diagnosis of animal coccidioses involves e.g. SPORULATION of
oocysts concentrated from fresh faeces.
[Identification of Eimeria spp: Book ref. 7, pp. 730. Identification of coccidia: Book ref. 18, pp. 8091. Coccidian
pathogenicity: Book ref. 18, pp. 287327. Pathology, lab. diagnosis, and therapy in cryptosporidiosis, isosporiasis, sarcosporidiosis and toxoplasmosis: Book ref. 118, pp. 211236.]
coccidium An individual, or a particular strain, of an organism
of the suborder EIMERIORINA.
coccobacillus A bacterial cell intermediate in morphology
between a COCCUS and a BACILLUS.
Coccodiscus See RADIOLARIA.
coccoid More or less spherical: cf. COCCUS.
coccoid bodies Thin-walled coccoid forms which develop from
the helical or vibrioid cells in old cultures of e.g. Aquaspirillum,
Campylobacter and Oceanospirillum spp; their formation is
enhanced by treatment with mitomycin or UV light. Coccoid
bodies resemble sphaeroplasts but are resistant to osmotic lysis;
the majority are apparently viable, germinating to form normal
cells when transferred to a fresh medium. (cf. MICROCYST.)
coccolith A calcified scale, generally measuring a few micrometres or less in diam., present on the cell surface in certain
cells of the COCCOLITHOPHORIDS. Coccoliths contain crystals of
calcite either of a single type (in holococcolithis) or, more
commonly, of different shapes and sizes (in heterococcoliths);
coccoliths are often elliptical in shape (but may be round,
polygonal, etc) and they commonly exhibit intricate patterns
and ornamentations which are species-specific. The coccoliths
of present-day coccolithophorids form a significant proportion
of some deep-sea oozes; however, coccolithophorids were even
more abundant in previous geological ages, particularly in the
Cretaceous, and the coccoliths of these organisms are major
constituents of Mesozoic (Jurassic and Cretaceous) and Cenozoic
chalks and marls. Coccolith morphology apparently changed
rapidly over the ages, making fossil coccoliths useful markers
in the biostratigraphy of sedimentary rocks [Book ref. 136,
from Naja haje can also give rise to a C3 convertase but not to
a C5 convertase. Unlike C3b, CVF is not inactivated by Factors
I and H; it therefore forms a C3 convertase which is not subject
to regulation.
cobweb disease A MUSHROOM DISEASE caused by Hypomyces
rosellus; it can be controlled e.g. by BENOMYL or PROCHLORAZ
[PP (1983) 32 123131].
cocarboxylase See THIAMINE.
coccal Pertaining to a COCCUS.
cocci See COCCUS.
coccidia The common name for protozoa of the suborder EIMERIORINA.
Coccidia (1) A subclass of protozoa (class Telosporea) later
incorporated, with the TOXOPLASMEA, in the subclass COCCIDIASINA. (2) A subclass of protozoa (class Sporozoea [JP (1980)
27 3758]) equivalent to the COCCIDIASINA.
Coccidiascus A genus of yeasts (family METSCHNIKOWIACEAE).
Cells: spherical to ovoid (515 m diam./length), with a large
vacuole and nucleus; neither pseudomycelium nor mycelium is
formed. C. legeri (sole species) occurs as a parasite in intestinal
epithelial cells of Drosophila spp; it has not been cultured in
vitro. [Book ref. 100, pp. 123124.]
Coccidiasina A subclass of protozoa (class SPOROZOASIDA) parasitic mainly in vertebrates but also in invertebrates. In members
of this subclass the mature gametocytes typically occur intracellularly in the host (cf. GREGARINASINA). Orders: Agamococcidiorida, EUCOCCIDIORIDA, Protococcidiorida.
coccidiasis Any subclinical or very mild infection with a coccidian parasite as distinct from clinical COCCIDIOSIS.
Coccidioides A genus of fungi (class HYPHOMYCETES); C. immitis
is a saprotroph in desert soils in hot, arid regions of the American
continent, and is the causal agent of COCCIDIOIDOMYCOSIS. In
mammalian tissues it occurs mainly as multinucleate, thickwalled, spherical (ca. 2080 m) cells (spherules or sporangia).
The spherule protoplasm divides into multinucleate protospores
and then into uninucleate sporangiospores (endospores) which
are released on rupture of the spherule wall and develop
into new spherules. C. immitis grows readily on various types
of media, forming a mycelium which fragments into barrelshaped arthroconidia which are highly infective and very easily
dispersed by air currents.
coccidioidin Any antigenic preparation derived from Coccidioides immitis and used in a diagnostic SKIN TEST for COCCIDIOIDOMYCOSIS.
coccidioidomycosis (San Joaquin Valley fever; desert fever) A
disease of man and animals caused by Coccidioides immitis; it
occurs in hot, arid regions of the American continent. Infection
usually occurs by inhalation of wind-borne spores (especially
arthroconidia); person-to-person transmission does not occur.
Infection may be asymptomatic or may result in an acute,
self-limiting respiratory disease resembling a common cold or
influenza often with severe chest pain. Rarely, mycetomas
(fungus balls) may develop in the lungs. Less common
symptoms include joint pains (desert rheumatism) and/or skin
lesions. The primary infection occasionally leads to progressive,
often fatal, disseminated disease (coccidioidal granuloma) with
lesions in e.g. skin, joints, meninges. Lab. diagnosis: serological
tests; SKIN TESTS using COCCIDIOIDIN or SPHERULIN; demonstration
of the fungus by histology, culture and/or animal inoculation.
Treatment: ketoconazole, amphotericin B. [Book ref. 25.]
coccidiosis Any disease of man and other animals caused by
protozoa of the suborder EIMERIORINA. Coccidioses are typically
contracted via the oral route and may involve the intestinal
176
codon bias
as four different RNA species. Two RNAs designated RNA1 small or RNA-1 fast (246 nucleotides) and RNA-2 small or
RNA-2 fast (492 nucleotides) occur in infected palms during
the early stages of cadang-cadang disease; later, two additional
RNAs RNA-1 large or RNA-1 slow (287 nucleotides) and
RNA-2 large or RNA-2 slow (574 nucleotides) appear and
eventually predominate. The RNA-1 small is regarded as the
unit CCCV RNA; the other three RNAs are apparently derived
from RNA-1 small by sequence duplication. [Nature (1982) 299
316321.]
coconut hartrot See HARTROT.
coconut lethal yellowing A YELLOWS disease of the coconut palm
caused by an MLO. The disease is controlled, commercially, by
the use of oxytetracycline hydrochloride.
coconut palm rhinoceros beetle (biological control) See BACULOVIRIDAE.
co-conversion (mol. biol.) See RECOMBINATION.
codecarboxylase See PYRIDOXINE.
coding strand A term which (like non-coding strand) is frequently used with opposite meanings by different authors. Originally, the term was generally used to refer to that strand of a
gene which acts as the template on which mRNA is synthesized
during transcription the strand whose sequence is complementary to that of mRNA. Currently, there appears to be a consensus
for the opposite meaning, i.e. that strand of a gene which is not
transcribed (i.e. not used as a template) and whose sequence is
homologous to that of mRNA. (Even so, given the confusion
present in the literature, it may be wise to define the term, in
relation to mRNA, whenever it is used.) The coding strand is
also called the sense strand or the plus (+) strand.
The non-coding strand of a gene (which is complementary to
the coding strand) is thus the template strand; it is also called
the antisense strand or the minus strand.
Interestingly, a certain gene in the fruitfly (Drosophila) has
been shown to contain protein-encoding information in both of
the strands [Nature (2001) 409 1000].
Codium
A genus of siphonaceous green seaweeds (division CHLOROPHYTA). The thallus is terete and dichotomously
branched; it is composed of a colourless central medulla of
interwoven filaments from which arises a surrounding layer of
inflated green branchlets (utricles). Anisogametes are produced
in the utricles; these are initially non-motile, later becoming
biflagellate. (See also CELL WALL; ELYSIA; NITROGEN FIXATION.)
codominant gene One of two (or more) genes which, when
present together, specify a phenotype unlike that specified by
either (or any) of the genes individually.
codon See GENETIC CODE.
codon bias In the expression of a heterologous (i.e. foreign)
gene (e.g. a mammalian gene in Escherichia coli): inefficient
translation due to the presence of certain codon(s) for which the
host cell has insufficient numbers of the corresponding tRNA(s);
codon bias can be a problem e.g. when high-level expression
in E. coli is required from a heterologous gene containing
a high frequency of codons such as the proline codon CCC
and/or the arginine codon AGG codons which occur rarely in
homologous (E. coli ) genes. Attempts at high-level expression
of genes containing relatively high frequencies of codons that are
rare for the host cell may lead e.g. to slowing or termination
of translation and the degradation of mRNA. One solution to
the problem is to insert into the host cell extra (plasmid-borne)
copies of the relevant tRNA-encoding gene(s).
Codon bias may also arise as a result of a same-sense mutation
which replaces a common or routine codon with a synonymous
but infrequent codon (see SILENT MUTATION).
Codonella
for catalysis of redox reactions. (2) Any low-MWt, nonprotein organic molecule whether freely dissociable or firmly
bound necessary for the activity of a given enzyme.
coenzyme F420 See METHANOGENESIS.
coenzyme F430 See METHANOGENESIS.
coenzyme I NAD (q.v.).
coenzyme II NADP: see NAD.
coenzyme A (CoA) A coenzyme, derived from PANTOTHENIC ACID
(see figure), which functions as a carrier of acyl groups with
which it forms thioesters (CoA.S.CO.R). (Uncombined coenzyme A may be represented as CoA-SH or CoASH.) Acylcoenzyme A thioesters have a high free energy of hydrolysis and
are commonly involved in SUBSTRATE-LEVEL PHOSPHORYLATIONS.
coenzyme B See METHANOGENESIS.
coenzyme B12 See VITAMIN B12
coenzyme F See FOLIC ACID.
coenzyme M See METHANOGENESIS.
coenzyme Q See QUINONES.
coenzyme R Syn. BIOTIN.
cofactor (1) Any low-MWt, non-protein (organic or inorganic)
factor which is necessary for the activity of a given enzyme
(cf. COENZYME; PROSTHETIC GROUP). (2) (Syn. activator) Any
inorganic component (e.g. metal ion) necessary for the activity
of a given enzyme. (3) Any organic or inorganic factor necessary
for the activity of an enzyme or enzyme complex.
coffee The commercial preparation of coffee from ripe coffee
fruits (cherries) requires the removal of the sticky mucilaginous
mesocarp which surrounds the two beans in each fruit. This
may be achieved mechanically or chemically, but the preferred
method is by fermentation which also improves the quality
and appearance of the beans. The coffee fruits are pulped to
disrupt the skins and then allowed to ferment either under water
or dry. The mucilage is degraded both by enzymes in the
fruit itself and by microbial extracellular enzymes. (Commercial
preparations of mould enzymes have also been used.) Various
bacteria, yeasts and moulds are associated with the fermenting
coffee, the most important probably being pectinolytic species of
e.g. Bacillus, Erwinia, Aspergillus, Fusarium and Penicillium.
After the fermentation, the beans are washed, dried, blended,
roasted and ground before use. (cf. COCOA.)
coffee berry disease A disease of the coffee plant characterized
by sunken, anthracnose lesions on the berries; causal agent:
Colletotrichum coffeanum. [Review: Phytopathol. Paper number
20, March 1977.]
O
N
CH2
O
1
CH3 OH
OH
P
O
CH2
CH2
CH2
CH2
CH2
SH
CH3 H
pantothenic acid
P O
adenosine 3,5-bisphosphate
pantetheine 4-phosphate
COENZYME A (CoA-SH)
178
2-mercaptoethylamine
(= cysteamine)
cold-shock response
colchicine An alkaloid found e.g. in the meadow saffron
(Colchicum autumnale); the colchicine molecule consists of a tricyclic skeleton which includes an aromatic ring (substituted with
three methoxy groups) and a tropolone ring. At low concentrations colchicine can e.g. bind to TUBULIN and prevent the in vitro
or in vivo assembly of tubulin into MICROTUBULES; colchicine
can thus e.g. inhibit MITOSIS in mammalian, plant, and other
cells. (However, some complex microtubular structures e.g.
CENTRIOLES, and the ciliar and flagellar axonemes are normally resistant to colchicine.) The in vitro effect of colchicine
on microtubule assembly can be abolished e.g. by ultraviolet
radiation (which converts colchicine to lumicolchicine).
coffee diseases For diseases of the coffee plant (Coffea spp) see
e.g. COFFEE BERRY DISEASE, COFFEE RUST, FUSARIUM WILT, PHLOEM
NECROSIS, RED RUST.
coffee ringspot virus See RHABDOVIRIDAE.
coffee rust A COFFEE DISEASE caused by Hemileia vastatrix.
Yellowish spots, which become orange, appear on the undersides
of the leaves, corresponding dark patches appearing on the upper
surfaces; infected leaves are shed, and yields of berries are
greatly reduced.
cognac See SPIRITS.
cognate In (e.g.) immunology, a word commonly used to mean
corresponding or matching.
cognate help (linked recognition) (immunol.) The binding of a
helper T cell to an antigen which is also bound by a B cell; the B
and T cells are thus physically linked via the antigen. Such joint
binding of antigen is accompanied by contact between various
receptors and ligands on the two cells; this leads to activation and
proliferation of both types of cell and formation of antibodies
by the B cell. (See also ANTIBODY FORMATION.)
The determinant (epitope) bound by the B cell is sometimes
referred to as the hapten, that bound by the T cell as the
carrier terminology that derives from earlier haptencarrier
studies.
cohesive ends Syn. STICKY ENDS.
cointegrate The (circular) product of fusion between two circular replicons (e.g. two plasmids, or a plasmid and a bacterial
chromosome) mediated by a TRANSPOSABLE ELEMENT (TE). Cointegration may occur as a result of a transposition event between
a replicon containing a TE and one containing a target sequence
for that TE. The transposition is accompanied by duplication of
both the TE and a sequence at the target site: see entry TRANSPOSABLE ELEMENT. An alternative mechanism of cointegrate formation involves recA-dependent reciprocal recombination between
homologous TEs in each of two replicons. (Some authors reserve
the term cointegration for the transposition event only.) (See
also Tn3.)
(The term cointegrate has also been used for any product of
fusion between two replicons, regardless of the mechanism by
which fusion occurred.)
coital exanthema See EQUINE COITAL EXANTHEMA.
col factor See COLICIN PLASMID.
col plasmid See COLICIN PLASMID.
Colacium A genus of EUGLENOID FLAGELLATES. The organisms
differ from other euglenids in that they generally form dendroid
or palmelloid colonies; flagellated cells, when formed, resemble
those of EUGLENA. C. libellae overwinters in association with
damselfly nymphs, becoming established in the rectum of the
insect.
colanic acid A capsular heteropolysaccharide (the M antigen)
produced e.g. by strains of Escherichia coli and Salmonella.
K12 strains of E. coli produce colanic acid and form mucoid
colonies at 30 C but not at 37 C; certain mutants (lon or capR)
produce colanic acid and appear mucoid at 37 C.
Colanic acid consists of repeating trisaccharide units of
(-glucose-fucose-fucose-), the central fucose residue of each
unit carrying a trisaccharide branch (galactose-glucuronic acidgalactose-). Non-carbohydrate substituents (e.g. acetyl and pyruvyl groups) may be present, the nature and position of such
groups varying e.g. with strain.
[Organization of the E. coli K12 gene cluster responsible for
production of colanic acid: JB (1996) 178 48854893.]
Colcemid (trade name) DEMECOLCINE.
CH3O
NHCOCH3
CH3O
CH3O
O
OCH3
COLCHICINE
cold sore
during early exponential growth at 37 C in E. coli i.e. under
non-stress conditions [EMBO (1999) 18 16531659].)
The cold-shock response can also be triggered by certain
inhibitors of translation for example, the antibiotics chloramphenicol, erythromycin and tetracycline; this has suggested that
a decrease in translational capacity may be an important factor in the induction of the cold-shock response [Mol. Microbiol.
(1994) 11 811818].
cold sore (fever blister) (1) The lesion associated with labial
herpes (see HERPES SIMPLEX). (2) The recurrent thin-walled
vesicular mucocutaneous lesion associated with any of the
various forms of HERPES SIMPLEX.
cold stability factor See MICROTUBULE-ASSOCIATED PROTEINS.
cold water disease (peduncle disease; low temperature disease)
A FISH DISEASE affecting young salmonids below 10 C. The tail
and peduncle undergo slow progressive necrosis. Causal agent:
Flexibacter psychrophila (Cytophaga psychrophila).
ColE1 plasmid A small (MWt ca. 4.2 106 ), non-conjugative,
ccc dsDNA COLICIN PLASMID which is normally maintained in
the host cell at a copy number of ca. 1030.
In ColE1, DNA REPLICATION occurs by the CAIRNS MECHANISM.
Replication is initiated from a fixed origin and (in contrast to
chromosomal replication in Escherichia coli ) proceeds unidirectionally from the origin; it is not dependent on plasmid-encoded
proteins but requires the cells RNA polymerase, DNA polymerases I and III and components of the PRIMOSOME. The first
several hundred nucleotides of the leading strand are synthesized
by DNA polymerase I from an RNA primer synthesized by RNA
polymerase; subsequent DNA chain elongation is carried out by
DNA polymerase III.
Initiation of plasmid replication is regulated at the level
of primer formation. During the initiation process, two RNA
transcripts are synthesized, one on each DNA strand, at the
same region ca. 500 nt upstream from the origin (ori). The
transcript on the H strand (RNA II) can unless prevented
(see later) extend to the origin and give rise to a primer for
synthesis of the leading strand; the transcript on the L strand
(RNA I, 108 nt long) is complementary to the 5 terminal region
of RNA II and behaves as a trans-acting repressor of plasmid
replication.
According to a current model, the 5 end of RNA II is
synthesized as a free (single-stranded) transcript, but as the RNA
polymerase approaches ori the transcript and template form a
DNA/RNA hybrid; the RNA strand in this hybrid is cleaved by
RNASE H to form a free hydroxyl (OH) terminal suitable for
extension by DNA polymerase, i.e. the cleaved end of the RNA
transcript, at ori, functions as a primer. (Although RNase H is
essential for replication of ColE1 in vitro, its role in vivo has
been questioned [JB (1986) 166 143147].)
Whether or not a functional primer is formed from the RNA
II transcript, as described above, is influenced by several factors factors which, by regulating the initiation of replication,
determine the COPY NUMBER of the plasmid.
One regulatory factor is RNA I. RNA I and RNA II each
form several stem-and-loop structures which, because the two
transcripts are complementary, can undergo mutual base-pairing;
when this happens, it inhibits development of a functional primer
at the RNA/DNA hybrid in the ori region. (In vitro, RNA I can
inhibit primer formation only if it binds to RNA II some time
before the complete RNA IIDNA hybrid has been formed; once
the nascent RNA II transcript has reached a length of 360 nt
it becomes resistant to RNA I.) The hybridization of RNA I
with RNA II is facilitated/accelerated by a small protein (63
colicins
colicin L See COLICINS.
colicin M A colicin (see COLICINS) (MWt ca. 23000) which binds
to the TONA PROTEIN (= FhuA); it inhibits the synthesis of
PEPTIDOGLYCAN.
colicin N A pore-forming colicin (see COLICINS) MWt ca. 39000)
which binds to the OmpF protein.
colicin plasmid (col factor, or col plasmid) A PLASMID which
encodes one or more COLICINS. Some col plasmids (type 1)
are small, MULTICOPY PLASMIDS, while others (type 2) are
large, low-copy-number plasmids. The type 1 col plasmids
are non-conjugative; type 2 col plasmids are often conjugative
(see CONJUGATIVE PLASMID). Conjugative col plasmids occur in
various INCOMPATIBILITY (Inc) groups (e.g. ColV is an IncFI
plasmid, ColB-K98 is an IncFIII plasmid, and ColIb-P9 is an
IncIa plasmid). Some non-conjugative plasmids have been found
to exhibit incompatibility [e.g. incompatibility between ColE
plasmids: JGM (1986) 132 18591862].
Col plasmids contain three essential genes: (i) the colicin
structural gene (= activity gene); (ii) a gene encoding the
immunity protein (see COLICINS); and (iii) a gene encoding the
lysis protein. These genes are designated cdl (colicin D lysis
gene), cea (colicin E activity gene), cui (colicin U immunity
gene) etc.
In a population of colicinogenic bacteria only a small proportion of the cells is de-repressed for colicin synthesis; however,
the immunity gene is usually expressed constitutively so that
cells with repressed genes for the colicin and lysis protein are
protected from the given colicin produced by their derepressed
neighbours.
A col plasmid typically encodes only that type of immunity
protein which protects the host cell against the particular colicin
encoded by the plasmid. However, ColE9-J encodes two types
of immunity protein: one protecting against colE9 and one
protecting against colE5 [JGM (1986) 132 6171].
Transcription of col plasmids is repressed by the LexA protein
so that synthesis of colicins is promoted by those agents which
trigger the SOS SYSTEM.
colicin typing BACTERIOCIN TYPING with COLICINS.
colicin U A pore-forming colicin (see COLICINS) (MWt ca. 66300)
produced by Shigella boydii ; colicin U binds to sensitive cells
via the OmpA and OmpF proteins, and uptake occurs via the
TolABQR proteins [JB (1997) 179 49194928].
colicin V The designation of a bacteriocin (MWt 6000) which
acts by disrupting the membrane potential of sensitive cells [JB
(1984) 158 757759]; it is not inducible by conditions which
trigger the SOS system (cf. COLICINS), and at least some authors
now classify this bacteriocin as a MICROCIN [e.g. TIM (1998) 6
6671].
colicin X The designation of a small bacteriocin subsequently
classified as a MICROCIN.
colicin Y A recently isolated pore-forming colicin (see COLICINS) encoded by plasmid pCol-Let [complete coding sequence:
Microbiology (2000) 146 16711677].
colicinogenic Able to produce COLICINS.
colicinogenic plasmid Syn. COLICIN PLASMID.
colicins A category of high-MWt (2590 kDa) BACTERIOCINS
produced by colicinogenic bacteria of the family Enterobacteriaceae (e.g. Escherichia coli, Shigella boydii ) and active against
(sensitive) strains of the same family; most colicins are encoded
by plasmid genes (see COLICIN PLASMID), one exception being the
chromosomally encoded bacteriocin 28b a bacteriocin (similar to colicin L) produced by strains of Serratia marcescens.
A given colicin is associated with a cluster of three genes:
(i) the structural gene for the colicin; (ii) the immunity gene,
coliform
coliform In general: any Gram-negative, non-sporing, facultatively anaerobic bacillus which can ferment lactose, with acid
and gas formation, within 48 hours at 37 C. For water bacteriologists (in the United Kingdom), a coliform is defined as
any member of the family Enterobacteriaceae which grows at
37 C and which normally encodes b-galactosidase [for further
information see Report 71 (1994) HMSO, London (ISBN 0 11
753010 7)].
Escherichia coli is a typical coliform.
coliform mastitis See MASTITIS (b).
coliform test A test used to detect the presence of COLIFORM
organisms in e.g. water (see INDICATOR ORGANISM and WATER
SUPPLIES); the test was originally designed to reveal faecal
contamination (hence the designation faecal coliform test). In
the test, aliquots of sample are used to inoculate a number of
tubes (see MULTIPLE-TUBE METHOD), each of which contains e.g.
MACCONKEYS BROTH and a DURHAM TUBE; incubation is carried
out at 37 C. A positive test (i.e. lactose fermentation) is shown
by acidification (pH indicator) and gas production (Durham
tube). The most probable number of coliforms in the original
sample can be calculated from the number of positive tubes
and the use of statistical tables. The count thus obtained is
actually a presumptive coliform count because, in any given
tube, a positive result could be due to certain endosporeforming bacteria (which also ferment lactose and form gas);
this possibility is particularly important when testing chlorinated
water samples because spore-forming bacteria are more resistant
than coliforms to chlorine. Confirmation that each positive
result is, in fact, due to thermotolerant (= faecal ) coliforms
involves two further 24-hour tests at 44 C: the INDOLE TEST and
the EIJKMAN TEST.
s DISEASE.
coli-granuloma Syn. HJARRE
coliphage A BACTERIOPHAGE that infects Escherichia coli. (For
coliphage l, coliphage T4 etc see BACTERIOPHAGE l, BACTERIOPHAGE T4, etc.)
colisepticaemia A respiratory and septicaemic disease of poultry
caused by strains of Escherichia coli. Incidence of the disease
has increased greatly with the advent of modern intensive rearing
methods, and often occurs secondarily to e.g. poor ventilation,
vaccination of birds with live vaccines (e.g. live Newcastle disease vaccines), or various other respiratory diseases (e.g. AIR
SACCULITIS, AVIAN INFECTIOUS BRONCHITIS, NEWCASTLE DISEASE).
Infection occurs mainly via the respiratory tract; characteristic
post-mortem findings include fibrinous pericarditis and perihepatitis.
colistins See POLYMYXINS.
colitis Inflammation of the colon. (cf. ENTERITIS.) Colitis occurs
e.g. in certain infectious diseases (e.g. amoebic and bacillary
DYSENTERY; see also SHIGA TOXIN). Antibiotic-associated colitis
sometimes occurs when the normal bowel flora is suppressed
by broad-spectrum antibiotic therapy; this condition ranges from
mild diarrhoea to PSEUDOMEMBRANOUS COLITIS, and is commonly
due to growth and toxin formation by Clostridium difficile (an
organism normally rare in adults, but common in the bowel in
infants). C. difficile produces at least two distinct hydrophobic
protein toxins, A (an enterotoxin) and B (a cytotoxin) [JMM
(1984) 18 385391]; toxin A causes fluid accumulation in the
intestinal lumen (but not by activating adenylate cyclase cf.
e.g. CHOLERA TOXIN), and the B toxin disaggregates filamentous
actin in tissue culture cells [GE (1984) 86 1212 (abstr.)].
[Purification and properties of cytotoxin B: JBC (1986) 261
13161321.] Chemotherapy: e.g. vancomycin.
colitose (3,6-dideoxy-L-galactose) A sugar, first isolated from
Escherichia coli, which occurs in the O-specific chains
columella
macrophages which, among other functions, stimulates the
development of macrophages from precursor forms such as
monoblasts and monocytes.
Colorado tick fever An acute human disease caused by a
virus and transmitted by the tick Dermacentor andersoni ; it
occurs in the Rocky Mountain regions of the USA. Symptoms
include fever, leucopenia, headache and myalgia, but no rash;
CNS complications occasionally occur in young children. Wild
rodents (e.g. ground squirrels) may act as a reservoir of infection.
The causal agent has been regarded as an ORBIVIRUS, but has
been shown to contain 12 dsRNA molecules [Virol. (1981) 112
361364] and may thus represent a distinct taxonomic group.
colostrum A secretion of the mammary gland produced before
lactation proper; it contains e.g. immunoglobulins (mainly IgA
and IgG). In man, the immunoglobulin content of colostrum is
relatively low, but in some animals e.g., ruminants (in which
immunoglobulins do not cross the placenta) large amounts are
normally present. (See also PASSIVE IMMUNITY.)
colour-breaking (breaking) The development of VARIEGATION in
flower petals; colour-breaking may occur as a result of virus
infection (e.g., in tulips infected with tulip breaking virus, a
member of the POTYVIRUSES). Flowers affected in this way are
often prized for their attractive appearance.
Colour Index (CI) A comprehensive reference publication on
dyes and pigments published by The Society of Dyers and
Colourists, Bradford, Yorkshire BD1 2JB, England. It consists
of a number of volumes which are periodically updated.
coloured field illumination Syn. RHEINBERG ILLUMINATION.
colourless sulphur bacteria Those non-photosynthetic SULPHUR
BACTERIA which obtain energy by the oxidation of sulphur and/or
reduced inorganic sulphur compounds (e.g. sulphide); although
referred to as colourless, some strains can exhibit pigmentation
owing to their content of cytochromes. The colourless sulphur
bacteria include e.g. species of Beggiatoa and Thiobacillus.
[Ecology of colourless sulphur bacteria: Book ref. 115, pp.
211240.]
Colpidium A genus of ciliates (order HYMENOSTOMATIDA) which
occur e.g. in freshwater habitats containing decomposing organic
matter. Cells: ovoid or reniform, ca. 50150 m, with uniform
somatic ciliature and a single macronucleus, micronucleus and
contractile vacuole. In C. colpoda (at least) asexual reproduction
occurs within a cyst.
Colpoda A genus of soil and freshwater ciliates (order COLPODIDA). Cells: typically reniform, ca. 40120 m in length, with
uniform somatic ciliation; the cytostome is lateral. C. steini is a
small species, ca. 2060 m, with a conspicuous tuft of cilia (the
beard) projecting from the region of the vestibulum. Food consists of other protozoa, algae and bacteria. Asexual reproduction
occurs within CYSTS in which four or more individuals may
be formed.
Colpodida An order of protozoa (subclass VESTIBULIFERIA) in
which the vestibular ciliature tends to be highly organized. Cysts
are common. The organisms are typically free-living, sometimes
associated with molluscs. Genera: e.g. COLPODA, Woodruffia.
Colpomenia See PHAEOPHYTA.
Colsargen See SILVER.
Columbia SK virus See CARDIOVIRUS.
columella An axial or central, unicellular or multicellular structure within a fruiting body in certain fungi and in certain slime
moulds of the MYXOMYCETES; in some cases it is simply an extension of the sporangiophore into the cavity of a sporangium, while
in others it may be a spherical, conical or cylindrical structure
extending upwards from the base of a sporangium. Although
column fermenter
(T. brevifaciens); affected plants show severe stunting and
chlorotic flecks on the leaves. (cf. KARNAL BUNT; see also CEREAL
DISEASES.)
common cold An acute disease of the upper respiratory tract in
man; the causal agent may be any of a range of viruses usually
a rhinovirus, coronavirus, influenza virus (type A, B or C),
parainfluenza virus (types 14) or human respiratory syncytial
virus. Incubation period: usually ca. 4872 hours. Symptoms
typically include coryza and nasal obstruction, sore throat,
cough, sneezing, but little or no fever. Direct contact may
be an important mode of transmission of rhinoviruses [AIM
(1978) 88 463]; the other viruses are probably transmitted
mainly by aerosols (see DROPLET INFECTION). Transmission of
rhinoviruses can be interrupted (experimentally) by the use of
virucidal (citric acid-treated) paper handkerchiefs [JID (1986)
153 352356]. Colds are usually self-limiting, but occasional
complications include e.g. OTITIS MEDIA, PNEUMONIA or SINUSITIS.
(cf. INFLUENZA.) [Review: Lancet (2003) 361 5159.]
common fimbriae Type 1 FIMBRIAE.
common pili (1) Syn. FIMBRIAE. (2) Syn. Type 1 fimbriae.
common scab (of potato) See POTATO SCAB.
communicable disease Syn. INFECTIOUS DISEASE.
comoviruses (cowpea mosaic virus group) A group of PLANT
VIRUSES in which the bipartite positive-sense ssRNA genome
is encapsidated in (separate) icosahedral particles; both parts
are necessary for infection. Most comoviruses cause systemic
mosaic or mottling and stunting occasionally with wilting,
necrotic ring formation, etc. in various plants, including e.g.
cowpea (Vigna unguiculata), beans, red clover etc; the host range
of individual members is narrow. Most comoviruses are transmitted by leaf-feeding beetles, particularly of the Chrysomelidae
(e.g. Cerotoma and Diabrotica spp); seed transmission occurs
in some comoviruses, and mechanical transmission can occur
readily under experimental conditions. Type member: COWPEA
MOSAIC VIRUS (SB isolate). Other members: e.g. cowpea severe
mosaic virus, quail pea mosaic virus, red clover mottle virus,
squash mosaic virus. (cf. BROAD BEAN WILT VIRUS.)
ComP See QUORUM SENSING.
compact colony-forming active substance See CCFAS.
comparative single intradermal tuberculin test (comparative
test; single intradermal comparative tuberculin test) (vet.) A
form of TUBERCULIN TEST, applied to cattle, in which two
intradermal injections are given (on a single occasion cf.
STORMONT TEST) at different sites on the same side of the neck;
PPD derived from Mycobacterium bovis is injected at one site,
PPD derived from M. avium is injected at the other site. After
72 hours any increase in skin thickness at the injection sites
is measured. If the response to PPD from M. bovis (increase
in skin thickness) is greater than that to PPD from M. avium
by a certain minimum amount then the animal is designated a
reactor. A positive reaction to PPD from M. avium together
with a negative reaction to PPD from M. bovis suggests contact
with M. avium and/or mycobacteria other than M. bovis.
The use of a defined antigen (ESAT-6), compared with PPD,
has been associated with lower sensitivity but higher specificity
[VR (2000) 146 659665].
comparative test (vet.) Syn. COMPARATIVE SINGLE INTRADERMAL
TUBERCULIN TEST.
comparator See WATER SUPPLIES.
compatibility (1) (of plasmids) See PLASMID. (2) (in fungal sexuality) The ability, or otherwise, of a given cell or thallus to
interact sexually with itself and/or with other cells or thalli of
the same species. In general, the genetic constraints on mating increase, both in number and complexity, from the lower
complement fixation
Complement fixation can be triggered in various ways, the
type of trigger determining which pathway is followed; four
pathways are shown in the figure.
(a) Classical pathway. This pathway is activated e.g. when
antigens bind to COMPLEMENT-FIXING ANTIBODIES in the presence
of complement. When such binding occurs, sequentially activated components may bind at or near the antigenantibody
complex; according to the antigen involved, this may result in
e.g. phagocytosis of the antigenantibody complex or, if a cellsurface antigen is involved, it may lead to cell lysis (see later).
The cascade of reactions which occur in the (antigen-triggered)
classical pathway is as follows.
The sequence is triggered when two or more subunits of C1q
(in the complement C1 molecule) bind to the FC PORTION of
antigen-bound IgG or IgM antibodies. Such binding (dependent
on calcium ions) activates the C1r component of C1 which, in
turn, activates the C1s component. C1s has serine protease and
esterase activity.
(Note that antibody-independent activation of C1 can be
promoted by certain non-specific activators e.g. C-reactive
protein (an ACUTE-PHASE PROTEIN) and various proteases.)
Activated C1s cleaves C4, forming C4a and C4b; as one
molecule of C1s can cleave many molecules of C4, this
reaction provides initial amplification. C4b molecules can bind
to bacterial or other surfaces; like C3b (see later), C4b is an
OPSONIN: C4b-coated cells or particles bind (via C4b) to the
CR1 receptor on the surface of phagocytes.
Surface-bound C4b may also bind C2. C2 is cleaved (in a
process involving C1s) to C2a and C2b; the complex formed
between the larger fragment, C2a (referred to as C2b in some
sources), and C4b (C4b2a) is a C3 convertase: an enzyme
which cleaves C3 to C3a and C3b (this being a major phase
of amplification in the complement cascade). (A low level of
C3 cleavage normally occurs spontaneously (C3 tickover) but
the resulting fragments are rapidly degraded.)
C3a is an ANAPHYLATOXIN.
C3b is an important OPSONIN, promoting e.g. the phagocytosis
of pathogens (IMMUNE ADHERENCE); C3b-bound antigens bind
(via C3b) to CR1 receptors on phagocytes.
C3b can also form a complex with C3 convertase: C4b2a3b;
this complex is a C5 convertase, i.e. it cleaves C5 into the small
fragment C5a and a larger fragment, C5b.
C5a is an ANAPHYLATOXIN and a chemoattractant for phagocytes (e.g. neutrophils).
C5b, C6 and C7 form a complex (C5b67) which binds to cell
membranes typically at the site of the initial triggering event.
Component C8 binds to the complex; this promotes polymerization of a number of C9 molecules within the membrane the
C9 molecules forming a pore or channel which, in some types of
cell (or even LIPOSOMES), can lead to lysis (immune cytolysis).
C5b678 and the C9 molecules collectively form the so-called
membrane attack complex, MAC. (Even in the absence of C9,
the complex C5b678 can bring about slow lysis e.g. in erythrocytes.)
For certain pathogens (e.g. trypanosomes), MAC-inflicted
damage can be lethal. In Gram-negative bacteria, pores formed
by the MAC in the OUTER MEMBRANE can promote cell lysis by
giving LYSOZYME access to cell-wall peptidoglycan; thus, e.g. a
Gram-negative bacterium on the conjunctiva would be at risk of
lysis because the tear film normally contains both complement
and lysozyme.
Sometimes, C5b67 binds to a cell other than that which
triggered the cascade; MAC-inflicted lysis in such a cell is called
fungi, through the ascomycetes, to the basidiomycetes. HOMOTHis common in all the major groups of fungi. Bipolar
HETEROTHALLISM occurs in some lower fungi (e.g. species of
Mucor and Rhizopus), in many ascomycetes (including e.g. Saccharomyces), and in many of the rust and smut fungi. Tetrapolar
heterothallism occurs in a number of basidiomycetes including
e.g. Schizophyllum commune and Ustilago maydis. (See also
MATING TYPE and PARASEXUAL PROCESSES.)
compatible (plant pathol.) Refers to a plantpathogen interaction which results in the development of disease in the plant.
(cf. INCOMPATIBLE.)
compatible solute Any low-MWt compound which, when
present intracellularly in high concentration, is compatible
with metabolism and growth. Compatible solutes involved in
OSMOREGULATION include: L-glutamate, GLYCEROL, ISOFLORIDOSIDE, MANNITOL, L-proline, glycine betaine [in Escherichia coli :
FEMS Reviews (1994) 14 320; in Staphylococcus aureus:
Microbiology (1994) 140 31313138], and certain sugars.
compensation level See PHOTIC ZONE.
competence See TRANSFORMATION (1).
complement (C or C ; historical syn. alexin or alexine) (immunol.)
A group of functionally related proteins present in normal
plasma, tissue fluids and the (freshly isolated) serum of
vertebrates. (In serum, the activity of complement is abolished
by exposure to room temperature for a few days, by heating to
56 C for 30 minutes, or by the action of chelating agents such
as EGTA or oxalate.) When activated, the complement system is
responsible for a number of important physiological activities
(see e.g. COMPLEMENT FIXATION).
Before activation, many of the components exist as proenzymes and/or inactive forms (cf. FACTOR D) which, on activation,
complex with, or act on, other components to form physiologically active entities.
In man, complement consists of nine numbered components
(C1C9, MWts ca. 80000200000) together with various proteins involved e.g. in stabilization or control functions: see e.g.
FACTOR B; FACTOR D; FACTOR H; FACTOR I; PROPERDIN and S PROTEIN. Component C1 is a complex macromolecule which consists
of three parts: C1q, C1r and C1s; C1q itself consists of a bundle
of six elongated subunits, and the macromolecule as a whole
depends on Ca2+ for its structural integrity.
Gene-based deficiencies in the complement system are associated with various adverse effects which depend e.g. on the
particular component(s) involved. One important role of complement is the removal of immune complexes (via the liver),
and deficiencies in C1, C4 and C2 may give rise to forms of
disease reflecting the accumulation of such complexes. A deficiency in C3 (with reduced capacity for opsonization) may result
in recurrent infections. A deficiency in MBL (lectin pathway) is
associated with increased susceptibility to infection in children.
Deficiencies in C5C8 generally cause increased susceptibility
to infection particularly with Neisseria.
complement activation Syn. COMPLEMENT FIXATION.
complement fixation (complement activation) Activation of the
COMPLEMENT system, i.e. promotion of the sequence (cascade)
of reactions in which various components of complement are
activated in turn. In vivo, complement fixation is involved
e.g. in certain immune responses and in INFLAMMATION; in
vitro it provides a sensitive system for various COMPLEMENTFIXATION TESTS. (Complement fixation is sometimes referred
to as complement inactivation an allusion to the fact that
components of complement are used up during fixation.)
ALLISM
185
complement fixation
CLASSICAL
LECTIN
ALTERNATIVE
C4
C4, C2
MBL
MASPs
C3b
LPS etc.
C1agab
C4b
C3bB
C2
C4b2a
amplification loop
factor B
factor D
properdin
PC3bBb
(C3 CONVERTASE)
C2a
factor I
(in plasma)
(C3 CONVERTASE)
C3
C3
C3b
C3b
C3b
C3bi
C4b2a3b
P(C3b)2Bb
(C5 CONVERTASE)
C5
(C5 CONVERTASE)
C5b
C6
C5b6
C7, 8, 9
C5b6789
COMPLEMENT FIXATION: four pathways (simplified scheme; see text). C1, C2 etc. denote particular components of the complement system;
a and b denote fragments of components produced by enzymic cleavage during the activation process. For clarity, the diagram does not
show all the cleavage products; for example, C4 is cleaved to C4a and C4b, but only the C4b fragment is considered here. Dotted lines
indicate those cases in which a given complex or component acts enzymically to cleave certain components of the system.
Reproduced from Bacteria 5th edition, Figure 11.1, page 292, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
C1INH), which inhibits initial activation of the classical pathway, and FACTOR I, which cleaves C3b to an inactive form,
C3bi. (C3bi, although inactive in the cascade, can nevertheless behave as an opsonin binding e.g. to the CR4 receptor
on macrophages.) Other regulatory factors are involved in the
control of the alternative pathway (see later).
(b) Alternative pathway. In evolutionary terms, this pathway is
apparently older than the classical pathway. In man, fixation via
the alternative pathway is initiated by e.g. bacterial LIPOPOLYSACCHARIDES, rabbit (but not sheep) erythrocytes, aggregates of
complementation test
lysed indicates the amount of free (unfixed) complement remaining. Practice: to detect or quantify e.g. a given antibody in a
sample of serum, SERIAL DILUTIONS of the INACTIVATED SERUM
are prepared, and known, fixed quantities of COMPLEMENT and
antigen are added to each dilution; the quantity of complement
added (determined by titration) should be sufficient to cause
lysis of ca. 90% of the erythrocytes in the haemolytic system
when no complement-fixation has occurred. Incubation is carried out for ca. 18 hours at ca. 4 C. (Low-temperature incubation
is used because some components of complement are labile at
room temperature.) A fixed volume of the haemolytic system
is then added to each dilution, and the whole is incubated for
1530 min at 37 C; the test dilutions are then left at ca. 4 C to
permit non-lysed erythrocytes to settle. In any given dilution, the
extent of haemolysis will be inversely proportional to the extent
of complement fixation in that dilution. If maximum haemolysis
is observed in the lowest serum dilution (i.e. the highest serum
concentration) the test is negative i.e. the serum contains no
detectable antibody. In a positive test, no haemolysis occurs in
(at least) the lowest serum dilution; a test may be regarded as
positive either (i) when no haemolysis has occurred in a specified number of serum dilutions (e.g. all dilutions up to 1:8 or
1:16 initial serum dilution), or (ii) when an increase in the titre
of complement-fixing antibodies is recorded in a second serum
sample taken some time after the first.
In all CFTs, controls are essential e.g. to check that the test
system is functioning correctly and to preclude false-positive
interpretations based on the effects of ANTICOMPLEMENTARY
substances.
complement-fixing antibodies Antibodies which fix or activate COMPLEMENT when they combine with their homologous
antigens. IgG (subclasses 1 and 3) and IgM can bring about
complement fixation via the classical pathway; aggregates of
IgA (subclasses 1 and 2) can activate the alternative pathway.
(See also FC PORTION.)
complement receptor 1 See CD35.
complementarity-determining regions (immunol.) Those HYPERVARIABLE REGIONS which occur at the surface of the
COMBINING SITE of an antibody.
complementary bases See BASE PAIR.
complementation The ability of a gene (or protein) to compensate for (i.e., to complement) a functional defect in a homologous gene (or protein) when present in the same organism or
cell. For example, a wild-type gene necessary for the synthesis of
a given amino acid may, when introduced into a mutant organism auxotrophic for that amino acid, complement the mutant
gene (by supplying an active form of the defective gene product) and restore the wild-type (prototrophic) phenotype. (See
also COMPLEMENTATION TEST; IN VITRO COMPLEMENTATION ASSAY;
NON-GENETIC REACTIVATION.)
complementation test A test used to determine whether or not
COMPLEMENTATION will occur in a cell with a given mutant
phenotype when another mutant genome, encoding the same
mutant phenotype, is introduced into that cell. The test involves
bringing together, into the same cell, the two (haploid) mutant
genomes (or a genome and part-genome see MEROZYGOTE) and
determining the resulting phenotype. The expression of a wildtype phenotype (a positive complementation test) indicates that
the mutations are in different genes in the two genomes, i.e.,
one wild-type form of each gene can be supplied by each of the
mutant genomes (intergenic or intercistronic complementation);
this indicates that at least two genes are involved in the
expression of that phenotype. (If the mutations were in the
complementing diploids
and the heap may be turned and mixed at intervals. The
pH may rise substantially (e.g. to 89), due e.g. to ammonia production, but later falls to ca. 67. After several days
the temperature may fall to ca. 3050 C and may remain at
this level for several weeks; during this stage fungi become
dominant. Initially, thermophilic members of the Mucorales
(e.g. Rhizomucor pusillus) develop; these are then replaced by
thermophilic hyphomycetes (e.g. Humicola spp, Thermomyces
lanuginosus) and ascomycetes (e.g. Chaetomium thermophilum).
Finally, basidiomycetes such as Coprinus cinereus (often accompanied by the zygomycete Mortierella wolfii ) become dominant
[Book ref. 39, pp. 263305]. During composting, most or all of
the free soluble substrates, much of the CELLULOSE, HEMICELLULOSES and PECTIC POLYSACCHARIDES, and some of the LIGNIN, are
degraded, and the loss in dry weight may reach 50% or more.
compound II See SIDEROPHORES.
compound ciliature Any form of somatic or oral ciliature which
involves a discrete group of cilia (several to many) acting as a
functional unit; examples: the CIRRUS, MEMBRANELLE, PARORAL
MEMBRANE and SYNCILIUM.
compound trichocyst Syn. FIBROCYST.
Compsopogon See RHODOPHYTA.
co-mutagenesis The generation of two or more mutations at
closely linked loci: see e.g. MNNG.
ComX See QUORUM SENSING.
con gene See OMP.
concanavalin A (con A; jack bean lectin) A mitogenic LECTIN
(tetrameric form: MWt 102000) from the jack bean, Canavalia
ensiformis; it can stimulate T cells and, if cross-linked (e.g.
by anti-con A antibody), B cells. Con A binds e.g. to terminal
a-D-mannopyranosyl and a-D-glucopyranosyl residues (binding
requires Ca2+ and Mg2+ ), and can thus agglutinate e.g. bacteria
whose cell wall TEICHOIC ACIDS contain a-linked glucosyl
substituents.
concatemer Two or more identical linear nucleic acid molecules
(e.g. copies of a viral genome) in tandem, i.e., covalently linked
end to end in the same orientation. (cf. CATENANE.)
concatenate (1) (verb) To form a concatenate (sense 2). (2)
(noun) Syn. CATENANE or CONCATEMER. (3) (adj.) Of e.g. spores:
formed in chains.
concentration exponent (of a disinfectant) See DILUTION COEFFICIENT.
concentric bodies (mycol.) Rounded or ellipsoidal intracellular
structures (ca. 300 nm diam.) which have a transparent core
surrounded by concentric layers of varying optical density; they
occur in almost all lichenized ascomycetes and in a few nonlichenized ascomycetes. Their origin and function are unknown.
Similar structures (concentric granules) are found in Allomyces
and related genera; these may play a role as septal pore plugs
[Mycol. (1987) 79 4454]. (cf. CELLULIN GRANULES.)
conceptacle (mycol.) A hollow structure within which spores are
formed e.g. a locule (see ASCOSTROMA).
conchate Having the shape of one-half of a bivalve shell.
Conchocelis stage See e.g. PORPHYRA.
concolorous Similarly coloured.
concomitant immunity Syn. PREMUNITION.
condenser (substage condenser) In a microscope: a system of
lenses which concentrates light and directs it onto the specimen
(see MICROSCOPY, Fig. 1). Correct adjustment of the condenser
conidium
conidiogenous cell See CONIDIUM.
conidioma Any plectenchymatous structure which bears conidia e.g. a pycnidium, sporodochium or synnema.
conidiophore A hypha which bears one or more conidiogenous
cells (see CONIDIUM). In e.g. some species of Colletotrichum,
setae (see SETA) can function as conidiophores.
conidiospore Syn. CONIDIUM.
conidium (mycol.) An asexually-derived, non-motile SPORE
formed in a blastic or thallic mode (see below) from a
specialized conidiogenous (i.e., conidium-producing) cell (cf.
SPORANGIOSPORE). Conidia are formed e.g. by many fungi
of the DEUTEROMYCOTINA and by a few lower fungi (e.g.
species of Bremia and Peronospora). The two basic modes of
conidiogenesis (conidium formation) are as follows.
Blastic conidiogenesis. An apical or lateral part of a conidiogenous cell expands and develops into a mature conidium,
becoming delimited from the parent cell by a septum. Such a
blastic conidium (= blastoconidium or blastospore) secedes (i.e.,
breaks away) from the conidiogenous cell by centripetal splitting of the septum (schizolysis) half the septum becoming the
base of the conidium, the other half forming the apex of the
conidiogenous cell. If the conidiogenous cell subsequently elongates from a basal growing region it is said to exhibit basauxic
development. (Cessation of hyphal tip growth see GROWTH
(b) preceding blastic conidiogenesis may depend on changes
in ion gradients across the envelope of the conidiogenous cell.)
Thallic conidiogenesis. A septum-delimited part of a hypha
becomes converted to a single, terminal or intercalary, conidium
(a holothallic conidium) or to a chain of conidia (arthric
conidia). (cf. ARTHROSPORE.) Secession of a terminal, holothallic
conidium commonly occurs by rhexolysis: the circumferential
splitting of the wall of the penultimate cell (which ruptures) a
little below the septum of the conidium; arthric conidia may
separate by rhexolysis (alternate cells being sacrificed) or by
schizolysis. [Formation and germination of fungal arthroconidia:
CRM (1986) 12 271292.]
There are various ways in which the conidiogenous cell can
produce a succession of conidia or give rise to a crop of
simultaneously formed conidia; some examples are given below.
(a) Ampullate development. The apex of the conidiogenous
cell becomes globose (ampullate) and gives rise, simultaneously, to a number of blastoconidia. Ampullate development
occurs e.g. in Gonatobotrys.
(b) Annellidic development. After the first, terminal blastoconidium has been delimited by a septum (and either before
or after its secession) a new wall is laid down on the inner
surface of the old wall in the distal region of the conidiogenous cell; this new, annular wall, in conjunction with the
apical septum, forms an inverted cup-like structure at the free
end of the conidiogenous cell. (The formation of the new wall
is referred to as enteroblastic proliferation of the conidiogenous
cell.) Subsequently, the cup-like structure expands to form the
next conidium; such a process, in which the new wall becomes
continuous with the conidial wall, is referred to as holoblastic conidial development. Septum formation then delimits the
second blastoconidium which (sooner or later) secedes by
schizolysis; the position of this septum is such that, following
secession of the blastoconidium, part of the new wall remains in
the conidiogenous cell, extending a little beyond the rim of the
old wall. Thus, after a number of blastoconidia have been produced, the conidiogenous cell (annellide) exhibits a succession
of bands (annellations) at the apical end, each annellation being
the remnant of a layer of wall formed inside the previous layer.
Coniocybe
TRANSPOSON-mediated conjugation is considered separately in
the entry CONJUGATIVE TRANSPOSITION.
Any of various plasmid-borne genes (and, in some cases,
chromosomal genes) may be transferred during conjugation;
such genes include those conferring resistance to antibiotic(s).
Conjugation occurs in both Gram-positive and Gram-negative
bacteria; however, as the process differs in Gram-positive and
Gram-negative species it is discussed under separate headings
for the two categories.
(i) Conjugation in Gram-negative bacteria. Much of the
information on this topic has derived from studies on the transfer
of the F PLASMID (q.v.), and other IncF plasmids, between strains
of Escherichia coli ; the following account is based largely on
this information. It is important to note that the general features
of the F plasmidE. coli transfer system are not common to all
transfer systems found in Gram-negative bacteria.
The stages of conjugation are outlined below, in sequence, on
the basis of current models and data.
Initial cellcell contact. The presence of a (plasmid-encoded)
pilus (see PILI) is believed to be essential for the donor phenotype. Moreover, different types of pilus mediate conjugation
under different physical conditions, and they may function
in different ways; for example, some types of pilus mediate
conjugation only on moist (but not submerged) solid surfaces
(e.g. agar plates), while others mediate conjugation either within
the liquid phase or on a solid surface (see PILI) [see also Book
ref. 177, pp 3359 (4245)].
In the F plasmidE. coli conjugal system, initial donorrecipient contact is believed to occur when the tip of the pilus binds
to a site on the surface of the recipient; the pilus is then believed
to retract so that the cells achieve wall-to-wall contact. Stable
cellcell contact, involving specific plasmid-encoded proteins,
is established after an initial period of unstable contact (during
which donor and recipient are easily separated by mild shearing
forces). (Mutant E. coli recipients defective in the OmpA protein
(see OMP) form unstable contacts with donor cells, although this
deficiency may be overcome by mating on a moist solid surface.)
(See also SURFACE EXCLUSION.)
An understanding of the initial donorrecipient interaction
would require a detailed knowledge of the structure and mode
of action of the pilus from initial contact to the putative
retraction. This information is currently unavailable; indeed,
the conjugal transfer of DNA, even in the well-studied F
plasmidE. coli system, and particularly in the initial stages of
cellcell contact, has been described as a black box [Mol.
Microbiol. (1997) 23 423429].
Some authors report that the region of contact between
donor and recipient is characterized by a specific, electron-dense
conjugational junction [JSB (1991) 107 146156; JB (2000)
182 27092715]. The composition of this electron-dense layer
is unknown but one suggestion is that, in F plasmid-mediated
matings, it may consist of, or contain, F-pilin (the subunit of
the F pilus) [Mol. Microbiol. (1997) 23 423429]; however,
results from recent studies on RP4-mediated matings indicated
that conjugational junctions are not composed of pilin [JB (2000)
182 27092715].
On establishment of effective cellcell contact, a mating
signal (nature unknown) promotes the mobilization of donor
DNA.
Mobilization and transfer of DNA. Mobilization is the process
in which (in at least some cases, including the F plasmid) a
single, specific strand of donor DNA is prepared for transfer to
the recipient.
conjugation
In the F plasmid, an essential prerequisite for mobilization is
the formation of a NICK at a specific site (designated nic), in
a specific strand, within the origin of transfer (oriT); nicking
occurs in that strand which is to be transferred to the recipient
(the T-strand). Nicking is mediated by an endonuclease (a
relaxase) that forms part of a so-called relaxosome (previously
called a relaxation complex). The relaxosome associated with the
F plasmid is a nucleoprotein complex consisting of the transfer
origin (oriT), the relaxase, and certain other proteins. (Relaxases
are encoded e.g. by the F plasmid traI gene, the traI gene of
plasmid RP4, and the nikA gene of Salmonella plasmid R64.) As
well as endonuclease activity, the TraI protein of the F plasmid
also has (ATP-dependent) helicase activity and is referred to as
helicase I.
Components of the relaxosome are assembled in a specific
order: TraI binds after the INTEGRATION HOST FACTOR and the
TraY protein [JBC (1995) 270 2838128386]. Recent studies
confirm that TraY is required for in vivo nicking [JB (2000) 182
40224027].
The relaxase is believed to mediate an ongoing cycle of
nicking and ligation at the nic site, i.e. nicking appears not to
be triggered by donorrecipient contact.
Following the mating signal in F plasmidE. coli systems, it
appears that the nicked strand enters the recipient in the 5 -to
3 direction. (Single-strand transfer in the 5 -to-3 direction is
believed to occur in at least some other cases.)
Transfer of the nicked strand from donor to recipient requires
that the strand be unwound from its complementary strand,
and this is thought to involve helicase I (TraI); if helicase I is
involved, and if it is immobilized in relation to the cell envelope,
then the unwinding of the transferred strand may provide energy
for strand transfer.
One early study indicated that the transferred strand could
pass through an extended pilus to the recipient [JB (1990) 172
72637264]. A later study which used video-enhanced lightmicroscopy and electron microscopy concluded that DNA is
transferred while donor and recipient are in close wall-to-wall
contact [JSB (1991) 107 146156].
The precise mode of transfer of DNA from donor to recipient
is not known. For F plasmid-mediated systems, it has been
postulated that the relaxosome may be coupled, via TraD, to
a transport apparatus (transferosome) consisting of a protein
complex located in the cell envelope at the base of the pilus.
In RP4-mediated mating, the transfer apparatus in the donor
may include a structure that bridges the cytoplasmic and outer
membranes [JB (2000) 182 15641574], although this was not
detected in another study on RP4-mediated mating [JB (2000)
182 27092715].
DNA synthesis in the recipient cell. When a cell receives the
transmitted strand of an F plasmid, a complementary strand
is synthesized to form a circularized dsDNA molecule; this
recA-independent process is called repliconation. Complementary strand synthesis apparently involves the recipients DNA
polymerase III and other host-encoded enzymes.
For certain IncI and IncP plasmids (e.g. ColIb, RP4), synthesis
of DNA in the recipient is initiated by a donor-plasmid-encoded
PRIMASE, i.e. during conjugation, primase, as well as ssDNA, is
transferred from donor to recipient. In such cases, DNA synthesis
is initiated from primers which are formed at various locations on
the transferred strand. [Plasmid DNA primases in conjugation:
Book ref. 161, pp 585603.] Matings with ColIb-P9 involve the
transfer, from donor to recipient, of molecules which include
the product of the sog gene, which has primase activity [EMBO
(1986) 5 30073012].
conjugational junction
pronucleus depends on its position within the cytoplasm; the
nucleus which survives is located in the cytostomal region
[JCS (1985) 79 237246].) The surviving pronucleus (= gonal
nucleus) divides mitotically to form a pair of gametic nuclei,
one of which passes to the conjugal partner and fuses with the
stationary nucleus to form a zygotic nucleus (= synkaryon).
Subsequently, mitotic divisions of each synkaryon lead to
the formation of four diploid nuclei in each conjugant the
conjugants by now having separated; two of the nuclei give
rise to two new micronuclei, while the other two form two new
macronuclei. During the first binary fission after conjugation,
the micronuclei (but not the macronuclei) undergo mitotic
division; each daughter cell receives one macronucleus and two
micronuclei thus restoring the normal nuclear constitution of
the species. In P. aurelia conjugation takes ca. 1218 hours.
[DNA synthesis, methylation and degradation during conjugation in Tetrahymena thermophila: NAR (1985) 13 7387.]
In peritrichs, two morphologically dissimilar conjugants are
formed: a female macroconjugant and a smaller, motile, ciliated
microconjugant which swims in search of, and fuses with, a
macroconjugant.
(See also AUTOGAMY and CYTOGAMY.)
(d) (mycol.) See e.g. MATING TYPE and PHEROMONE.
(2) (immunol.) The process of covalently linking two or more
species of molecule to form a hybrid molecule (a conjugate);
for example, a dye may be linked to a protein (as in fluoresceinconjugated antiglobulin), or glutaraldehyde may be used to link
two different antibodies to form a hybrid antibody [SAB (1984)
22 7378]. (See also CONJUGATE VACCINE.)
conjugational junction See CONJUGATION (1b)(i).
conjugative pili See PILI.
conjugative plasmid (1) (self-transmissible plasmid) As commonly used: a PLASMID which encodes all the functions needed
for its own intercellular transmission by CONJUGATION (sense 1b);
in e.g. the F PLASMID (q.v.) these functions include pilus formation (see PILI) and the formation of proteins involved in the
initial preparation of plasmid DNA for transfer. Such a plasmid may also bring about the mobilization of a (mobilizable)
NON-CONJUGATIVE PLASMID or the mobilization of the donors
chromosome. (cf. SEX FACTOR; see also ANDROPHAGE and PROMISCUOUS PLASMIDS.)
(2) According to some authors [ARG (1979) 13 99125
(105106)]: a plasmid which encodes e.g. pilus formation but
which may or may not be capable of mobilization; only if such
a plasmid is mobilizable is it self-transmissible.
conjugative transposition In bacteria: CONJUGATION mediated by
a conjugative transposon, i.e. independently of a conjugative
plasmid, the transposon being transferred from the donor cell
to the recipient cell. First reported in Gram-positive bacteria, it
is now well established in Gram-negatives (e.g. Bacteroides);
indeed, it may permit gene transfer between Gram-positives and
Gram-negatives [e.g. AEM (2001) 67 561568; AEM (2003)
69 45954603].
A model for Gram-positive conjugative transposition was as
follows. Contact between donor and recipient triggers excision of
the transposon in the donor, this involving a transposon-encoded
recombinase (product of gene int). Each end of the excised
transposon carries single-stranded host DNA called a coupling
sequence. The excised transposon then circularizes through basepairing (albeit mis-matched) between coupling sequences. A single
strand may be transferred to the recipient, the complementary
strand being synthesized in the recipient prior to insertion. Insertion
of the (double-stranded) transposon into the target site is neither
contagious hypovirulence
in a chemostat tend to be unstable at or near the maximum
growth rate.
In the turbidostat a culture normally grows at or near the
maximum growth rate, and all substrates are usually present in
excess; within certain limits, the concentration of biomass in the
turbidostat can be selected by the operator, and a steady state
is achieved by adjusting the dilution rate such that cell growth
is matched by the rate of loss of cells from the culture vessel.
Control of culture density (i.e. number of cells per unit volume)
may be achieved e.g. by a photosensitive device which monitors
the opacity of the culture and automatically adjusts the flow
rate; however, this method may suffer from inaccuracies due
e.g. to foaming and to wall growth (see later). Alternatively,
culture density can be controlled by monitoring other parameters
which are closely linked to specific growth rate e.g. pH (in a
pH-stat), CO2 evolution (in a CO2 -stat), or oxygen uptake.
In continuous culture, deviations from ideal (predictable)
operation are common. Such deviations may arise e.g. as a result
of the inability to achieve perfect (100%, instantaneous) mixing
of the inflowing medium with the culture fluid; imperfect mixing
may be indicated by a stable dilution rate which exceeds Dc .
Changes in the rate of agitation can affect the mean cell volume
of the cultured cells [JGM (1985) 131 725736]. Wall growth
(adherence to, and growth of, the cultured cells on the walls
of the culture vessel) may give an effect similar to (but usually
greater than) that of imperfect mixing. Another type of deviation
may occur when cells are cultured at low rates of growth; for
example, under carbon-limited conditions a major part of the
carbon source may be used to provide MAINTENANCE ENERGY
(thus giving a lower-than-predicted yield of biomass), while
under carbon-excess conditions the yield of biomass may be
greater than predicted owing to the accumulation of intracellular
reserve polymers (e.g. PHB). A different type of problem
involves the emergence of mutants during the (extended) periods
of culture an effect which can change the character of the
biomass if particular mutant(s) can outgrow the parent strain;
nevertheless, it is possible to take advantage of this effect e.g.
when it is desired to isolate mutants which synthesize more (or
more effective) enzyme(s) or which can take up the growthlimiting substrate more efficiently than can the parent strain.
continuous-flow culture Syn. CONTINUOUS CULTURE.
continuum model See CELL CYCLE.
Contophora Algae except members of the RHODOPHYTA. (cf.
ACONTA.)
contour-clamped homogeneous electric field electrophoresis
(CHEF) See PFGE.
contractile vacuole An osmoregulatory organelle, one or more
of which may occur in the cytoplasm in most freshwater
(and some saltwater) eukaryotic microorganisms (cf. PUSULE);
basically, it is a membrane-limited region which, under normal
environmental conditions, alternately fills with fluid (diastole)
and then discharges the fluid to the exterior (systole). During
diastole, the contractile vacuole may be fed by a surrounding
layer of small vesicles which appear to coalesce with the main
vacuole (as in amoebae), and/or depending on species it
may be fed by a system of collecting tubules which ramify
in the cytoplasm (forming the spongiome, = spongioplasm, =
nephridial network) and apparently drain areas remote from the
vacuole (a system characteristic of ciliates). In some protozoa
(e.g. Paramecium, Tetrahymena) discharge occurs at a fixed site
(pore) in the pellicle.
The mechanism of contractile vacuole activity is not known.
Systole may involve cytoplasmic turgor pressure; at least in
copy number
However, in effective concentrations, copper and certain of
its compounds are useful antimicrobial agents; toxicity to
microorganisms appears to reside in the cupric ion.
Copper sulphate has been used as an anti-algal agent in e.g.
swimming pools and as a constituent of various agricultural
antifungal agents (see e.g. BORDEAUX MIXTURE, BURGUNDY MIXTURE, CHESHUNT COMPOUND). Copper naphthenate is a greenish,
waxy solid, soluble in various organic solvents, which is used
as an antifungal preservative for e.g. cellulosic textiles. Copper
soaps are copper salts of certain fatty or oleoresinous acids (e.g.
copper stearate, copper tallate) which have antifungal activity
similar to that of copper naphthenate. Cuprammonium hydroxide is used in aqueous solution for rot-proofing fabrics. Cupric
ions are complexed by 8-HYDROXYQUINOLINE (one atom of copper to two molecules of 8-hydroxyquinoline) to form copper
8-quinolinolate (copper-oxine; copper oxinate) which is a highly
effective antifungal agent used e.g. in agriculture and as a preservative for textiles. (Copper compounds are not used in rubber
products since they catalyse the oxidation of rubber.)
copper 8-quinolinolate See COPPER.
copper soaps See COPPER.
co-precipitation (serol.) The precipitation of otherwise nonprecipitating molecules etc. as part of, or enmeshed with, an
immune complex.
Coprinaceae See AGARICALES.
Coprinus A genus of humicolous, lignicolous or coprophilous
fungi (AGARICALES, Coprinaceae) in which, in most species, the
lamellae undergo rapid autodigestion at maturity (see LAMELLA
and BASIDIOSPORE). (See also INK-CAP FUNGI.)
coproantibodies Antibodies produced by the intestinal mucosa
and found in the lumen of the gut; they are mainly of the
secretory IgA class.
Coprococcus A genus of Gram-positive, asporogenous, anaerobic bacteria which occur e.g. in the human gut; the organisms
ferment carbohydrates with the production of butyric and acetic
acids. Cells: cocci, occuring in pairs or chains. GC%: ca. 3942.
coprogen See SIDEROPHORES.
Copromyxa See ACRASIOMYCETES.
Copromyxella See ACRASIOMYCETES.
coprophilic (coprophilous) Refers to an organism which grows
preferentially or exclusively on or in animal faeces. For example,
certain fungi (e.g. species of Coprinus, Pilobolus and Sordaria)
grow more or less specifically on dung particularly that of
herbivorous animals.
co-protease (coprotease) A type of molecule which, acting nonenzymically, can promote autocatalytic cleavage of a protein; an
example is RecA in the SOS SYSTEM.
coprozoic Refers to e.g. protozoa which are COPROPHILIC.
copy-choice model See RECOMBINATION.
copy-mutant (copy-number mutant; cop mutant) A mutant PLASMID whose COPY NUMBER differs from that of the wild-type
plasmid. In copy mutants the copy number is usually higher
than that of the wild-type plasmid, but in some cases it is lower.
copy number (1) (of a bacterial plasmid) The number of copies
of a given PLASMID, per chromosome, in a cell; copy number
depends on the replication control system encoded by the
plasmid, on the strain or species of cell in which the plasmid
occurs, and on growth conditions. In plasmid-containing bacteria
in the exponential phase of growth, a given plasmid occurs with
a characteristic copy number; any perturbation in copy number
tends to be corrected by a rise or fall in the frequency of plasmid
replication. Mutations in a plasmid (and/or chromosome) may
give rise to a COPY MUTANT.
CoQ
velvety, exhibiting a number of dark bands concentric about the
region of attachment, while the lower surface is pale; basidiospores: cream-coloured, ca. 6 2 m. (See also WHITE ROT
and LIGNIN.)
corn oil test (for lipase) See LIPASE.
corn stunt disease A leafhopper-transmitted YELLOWS disease of
maize, characterized by stunting and leaf striping/discoloration,
caused by the MAIZE CHLOROTIC DWARF VIRUS or by certain
strains of Spiroplasma citri. [Proposal to regard the corn stunt
spiroplasmas as a distinct species, S. kunkelii : IJSB (1986) 36
170178.]
cornmeal agar A mycological medium. Essentially, cornmeal
(4% w/v) is heated in distilled water for 1 hour at 6065 C;
agar (1.5% w/v) is added to the filtrate, and the medium is
autoclaved. Cornmeal agar is used e.g. to demonstrate chlamydospore formation in Candida albicans which is reported to
be encouraged by the addition to the medium of Tween 80.
cornute Syn. ROESTELIOID.
Coronaviridae A family of pleomorphic, enveloped, nonsegmented ssRNA viruses which infect man, animals or
birds. One genus (Coronavirus) is currently recognized.
Members include AVIAN INFECTIOUS BRONCHITIS virus (IBV;
type species), human coronavirus (a causal agent of the
COMMON COLD), murine hepatitis virus (MHV), porcine
haemagglutinating encephalitis virus (see VOMITING AND WASTING
DISEASE), and porcine TRANSMISSIBLE GASTROENTERITIS virus;
probable members include e.g. coronavirus enteritis of turkeys
virus (= turkey bluecomb disease virus), and neonatal calf
diarrhoea coronavirus. Possible members include feline
infectious peritonitis virus (= feline coronavirus) and human
enteric coronavirus (a possible causal agent of human FOOD
POISONING).
Virion: ca. 75160 nm diam., consisting of a helical nucleocapsid surrounded by the envelope; characteristic club-shaped
glycoprotein projections (peplomers, spikes) 1224 nm long
extend from the outer surface of the envelope. Genome: positivesense ssRNA, MWt typically ca. 67 106 (8 106 has been
reported for IBV). The RNA is polyadenylated at the 3 end.
Proteins associated with the virion include (at least) S (spike),
M (membrane) and N (nucleocapsid). The virions are inactivated
e.g. by lipid solvents and by detergents.
Virus replication occurs in the host cell cytoplasm. In IBV,
6 subgenomic mRNAs (AF) are formed, all of which are 3 coterminal with the genomic RNA (a so-called nested set of
mRNAs); each 5 end has a common leader sequence (ca. 70
bases long) derived from the 5 end of genomic RNA [possible
mechanism: JGV (1986) 67 221228]. (MHV forms a nested
set of 7 subgenomic mRNAs, designated RNA1RNA7.) The
virions mature by budding through the endoplasmic reticulum
into vesicles.
[Molecular biology of coronaviruses: AVR (1983) 28 35
112.]
Coronavirus See CORONAVIRIDAE.
Coronie wilt Syn. HARTROT.
correction collar A part of a microscope objective lens which
is used to adjust the lens to work with cover-glasses of various
thicknesses.
corrinoids See VITAMIN B12 .
Corriparta subgroup See ORBIVIRUS.
corrosive sublimate See MERCURY.
cortex (1) Any of various external or outer layer(s) of a structure
or organism e.g. the outer differentiated tissue of certain
LICHENS; in ciliates cortex refers to the PELLICLE together with
the INFRACILIATURE. (2) See ENDOSPORE.
coryza
typically form shiny, greyish-black, entire colonies, 12 mm
at 24 hours, on bloodtellurite media; haemolysis is very
common. Each cell typically contains several metachromatic
granules. The ulcerans variety [Book ref. 46, p. 1831] (=
C. ulcerans) produces urease and gelatinase, and ferments
starch and trehalose as well as glucose, maltose and mannose;
haemolysis is common. Pyrazinamide is not hydrolysed. (See
also ULCERACIN 378.)
C. equi. See RHODOCOCCUS.
C. fascians. See RHODOCOCCUS. (See also FASCIATION.)
C. flaccumfaciens. See CURTOBACTERIUM.
C. glutamicum. A species which occurs e.g. in soil and
vegetable matter; certain strains are used for the industrial
production of GLUTAMIC ACID. C. glutamicum is nutritionally
fastidious; biotin is necessary for growth, and some strains are
reported to need B vitamins.
C. haemolyticum. See ARCANOBACTERIUM.
C. hydrocarboclastus. See CORYNECINS.
C. minutissimum. A species [incertae sedis: Book ref. 21,
p. 605] which is the causal agent of ERYTHRASMA; the organisms
ferment glucose, maltose, mannose, and usually sucrose [Book
ref. 46, p. 1831].
C. oortii. See CURTOBACTERIUM.
C. ovis. See C. pseudotuberculosis.
C. parvum. See PROPIONIBACTERIUM.
C. poinsettiae. See CURTOBACTERIUM.
C. pseudotuberculosis (formerly C. ovis). The causal agent
of pyogenic infections in e.g. cattle, horses and sheep (see e.g.
CONTAGIOUS PUSTULAR DERMATITIS (2), and ULCERATIVE LYMPHANGITIS). The organisms typically form yellow colonies; acid is produced from glucose, maltose and mannose, and urease is formed.
Some strains are haemolytic. Pyrazinamide is not hydrolysed.
C. pyogenes. See ACTINOMYCES.
C. renale. A species isolated e.g. from urinary tract infections
in cattle. Colonies are typically cream to yellow; glucose and
mannose (but not maltose) are fermented, and urease is formed.
Pyrazinamidase and caseinase are formed.
C. salmoninus. See RENIBACTERIUM.
C. ulcerans. See C. diphtheriae.
C. xerosis. A species which occurs e.g. on the conjunctivae
and in the throat in man; usually non-pathogenic, but cases
of endocarditis following aortic valve replacement have been
reported. Colonies are greyish; typically, glucose, maltose,
mannose and sucrose are fermented, and pyrazinamidase is
formed. Urease-negative.
corynecins Compounds analogous to chloramphenicol in which
the N-dichloroacetyl substituent is replaced with nonhalogenated acyl groups; corynecins have been isolated
from Corynebacterium hydrocarboclastus. (A type strain of
C. hydrocarboclastus has been shown to have the properties of
a species of Rhodococcus [JGM (1982) 128 25032509].)
coryneform (1) (club-shaped) Essentially rod-shaped with one
end thickened or bulbous. (2) A name applied, loosely, to
any Gram-positive, asporogenous, pleomorphic rod-shaped bacterium; as such it covers bacteria from a range of genera. (cf.
DIPHTHEROID.)
Coryneliales See ASCOMYCOTINA.
corynephage A BACTERIOPHAGE which infects Corynebacterium
spp. (See also DIPHTHERIA TOXIN.)
corynomycolic acids MYCOLIC ACIDS of Corynebacterium spp.
coryza Discharge from the nasal mucous membranes a symptom of e.g. the COMMON COLD and the prodromal phase of
MEASLES.
cos
cos See BACTERIOPHAGE LAMBDA; BACTERIOPHAGE P2; COSMID.
Coscinodiscus See DIATOMS.
Cosmarium A large genus of placoderm DESMIDS. The cells are
elliptical or angular in outline, with a deep sinus; the semicells
may be ornamented but lack prominent projections or spines (cf.
XANTHIDIUM). (See also SINGLE-CELL PROTEIN.)
cosmid A PLASMID into which has been inserted the cos site
of BACTERIOPHAGE LAMBDA. Cosmids can be used as CLONING
vectors for large fragments of DNA (e.g. ca. 2540 kb), and
have been useful e.g. in the construction of genomic libraries.
The use of a cosmid is shown diagrammatically in the figure.
(See also PHASMID.)
COSMID (diagrammatic). The cosmid (top) is a plasmid containing (i) a cos site (solid black square) from bacteriophage lambda, and (ii) the
cutting site (short vertical bar) of a RESTRICTION ENDONUCLEASE.
Cosmids are cut at the single restriction site, yielding linearized molecules with an internal cos site (top, left). Linearized cosmids are mixed
with DNA fragments (dashed lines) which have been cut by the same restriction enzyme.
Cosmids and fragments bind randomly via sticky ends, and in some cases a fragment will be flanked by two cosmids (centre). If, in such
a molecule, the distance cos-to-cos is approximately 4050 kb, then the coscos sequence is the right size for packaging into a phage
lambda head (the phage lambda genome is 48 kb). Enzymic cleavage at the cos sites (arrowheads) creates sticky ends, and packaging of
the recombinant molecule occurs, in vitro, in the presence of phage components.
The completed virions can inject their recombinant molecules into suitable bacteria. Within a bacterium the DNA circularizes, via the cos
sites, and replicates as a plasmid; its presence in the cell can be detected e.g. by the expression of plasmid-encoded antibiotic-resistance
genes.
Screening for specific sequences in cosmids is carried out in a way similar to that used for plasmid vectors.
Reproduced from Bacteria 5th edition, Figure 8.15, page 197, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
198
counting methods
amounts of slime are secreted over the body. Mortality may be
massive in fish hatcheries.
co-substrate See CO-METABOLISM.
cot death Syn. SUDDEN INFANT DEATH SYNDROME.
cotransduction The TRANSDUCTION of two or more donor genes
in the same transducing virion.
co-transfer (of plasmids) See CONJUGATION (1b) (i).
co-transport Syn. SYMPORT.
cotrimoxazole See FOLIC ACID ANTAGONIST.
cottage cheese See CHEESE-MAKING.
cotton anthocyanosis virus See LUTEOVIRUSES.
cotton blue Syn. METHYL BLUE.
cotton wilt Any VASCULAR WILT of cotton plants (Gossypium
spp). Common causal agents include Fusarium oxysporum f.
sp. vasinfectum (Frenching disease) and Verticillium dahliae.
cotton wool A fibrous, cellulosic material from seed coats of the
cotton plant (Gossypium). Non-absorbent cotton wool contains
substances (e.g. unsaturated fatty acids) inhibitory to certain
organisms; absorbent cotton wool has been treated with solvents
and bleached so that the inhibitory substances have been largely
or completely removed. Plugs of non-absorbent cotton wool are
often used as stoppers in tubes of bacteriological media. (See
also SWAB.) (cf. cotton wool substitute in the entry ALGINATE.)
cotton wool disease See COLUMNARIS DISEASE.
cottontail rabbit papilloma virus See PAPILLOMAVIRUS.
cotype Syn. SYNTYPE.
cou gene See GYRASE.
cough plate A method for isolating Bordetella pertussis from a
suspected case of WHOOPING COUGH. A plate of BORDETGENGOU
AGAR is exposed to droplet inoculation from the patients cough
and is then incubated and examined for growth of B. pertussis.
Many clinicians now use a pernasal swab (optimally, with an
ALGINATE tip) in preference to the cough plate method.
Coulter counter An instrument used for counting particles (cells,
spores etc) in a suspension. Essentially, it consists of two
chambers separated by a partition of (electrically) insulating
material which is perforated by a single hole of size similar
to that of the particles to be counted. Each chamber contains
an electrode. The sample is placed in one chamber and forced,
under pressure, into the other; during this transfer the suspension
acts as a conducting path (via the hole) between the two
electrodes. As each cell passes through the hole, it momentarily
decreases the electrical conductivity between the electrodes; this
momentary change in conductivity is recorded as a pulse by an
electronic counting circuit controlled by the two electrodes. The
cell count is indicated on a digital display. (See also COUNTING
METHODS.)
coumermycins A group of compounds structurally related to
NOVOBIOCIN. Coumermycin A1 inhibits ATP-dependent GYRASE
activity in the same way as NOVOBIOCIN, but is much more
effective both in vivo and in vitro.
Councilman body A cluster of hyaline, necrotic, eosinophilic
cells in the liver of an individual suffering from YELLOW FEVER.
counter-receptor (to a CAM) See CELL ADHESION MOLECULE.
counter transport Syn. ANTIPORT.
countercurrent immunoelectrophoresis (CIE) IMMUNOELECTROPHORESIS (used for only certain types of antigen) in which
antibodies and antigens (in separate wells in a gel strip) move
towards each other when subjected to the same electric field; the
antibodies move towards the cathode (see ELECTROENDOSMOSIS)
while the antigens because of their size, charge, and other
physico-chemical characteristics move towards the anode.
counterstain (1) A second, contrasting, stain used on a microscopical preparation with the object of staining those features
which have not taken up the first stain. (2) In the GRAM STAIN: a
stain used to stain those organisms or tissues which have been
decolorized. (3) In the AURAMINERHODAMINE STAIN: the solution of potassium permanganate used to eliminate background
fluorescence.
counting chamber (haemocytometer) An instrument used for
determining the total cell count, viable cell count, or spore count
etc. of a suspension of cells or spores (see COUNTING METHODS).
A typical counting chamber is illustrated on p. 200. A grid,
etched on the central plateau of the glass block, typically consists
of a square of side 1.0 mm divided into 400 squares, each
0.0025 mm2 ; the distance between grid and cover-slip may be
0.1 mm (as in the Thoma chamber) or 0.02 mm (as in the Helber
chamber). When the cover-slip is correctly positioned, Newtons
rings should be visible through those parts of the cover-slip
in contact with the glass shoulders indicating close contact.
The suspension is introduced (with a Pasteur pipette) into the
space between cover-slip and central plateau; the troughs should
remain empty. The cells are allowed to settle and are counted
under the microscope; since the volume between grid and coverslip is known, the count per unit volume can be calculated. For
viable cell counts, cells are subjected to VITAL STAINING.
(See also FACS.)
counting methods Methods for counting microorganisms may be
divided into two categories according to the type of organism
considered.
(a) Organisms other than viruses, viroids etc. The total number
of living and dead cells in a given volume (or on a given area)
of a sample is termed the total cell count; usually, total cell
counts refer to bacteria, spores or yeasts (single-celled organisms). A total cell count may be determined by direct (visual)
counting, i.e., by MICROSCOPY (see also COUNTING CHAMBER), or
by the use of electronic or other instruments (see e.g. COULTER COUNTER, NEPHELOMETRY, TURBIDIMETRY); both direct and
electronic methods may permit the counting of specific types of
cell e.g. by IMMUNOFLUORESCENCE microscopy and FACS (q.v.),
respectively. Liquid samples containing small numbers of cells
can be membrane-filtered (see FILTRATION) and the (stained) cells
counted in situ. (See also DEFT.) Cell numbers in a given suspension may be estimated by comparison with standard suspensions
(see BROWNS TUBES).
Viable cell count refers to the number of living cells (per
volume or area) in a given sample; viable cell counts usually
refer to single-celled organisms, and they can obviously include
only those organisms which are detectable by the particular
method used. A viable cell count may be determined in several
ways. (i) Direct examination, in a counting chamber, of a
sample stained with a vital stain (see VITAL STAINING) living
and dead cells being distinguished by their different reactions to
the dye. (ii) Statistical methods: see e.g. MULTIPLE-TUBE METHOD.
(iii) Colony counts: the number of viable cells in a sample (or
aliquot) is assessed from the number of colonies which develop
on incubation of a solid medium which has been inoculated
with the sample or aliquot; in such methods it is assumed that
each colony developed from a single cell. The selectivity of
the medium and the conditions of incubation may significantly
affect the number of viable cells which give rise to colonies. For
colony-counting methods see e.g. DIP-SLIDE METHOD, MILES AND
MISRAS METHOD, POUR PLATE, ROLL-TUBE TECHNIQUE and SPREAD
PLATE (sense 1).
Some types of cell tend to form clumps or to grow in chains
or filaments or in microcolonies. An accurate viable count of
such organisms cannot be obtained by the above methods, and
199
(a)
(b)
(c)
COUNTING CHAMBER (Thoma chamber). The instrument seen from one side at (a) consists of a rectangular glass block in which the
central plateau lies precisely 0.1 mm below the level of the shoulders on either side. The central plateau is separated from each shoulder by a
trough, and is itself divided into two parts by a shallow trough (seen at (b)). On the surface of each part of the central plateau is an etched grid
(c) consisting of a square which is divided into 400 small squares, each 1/400 mm2 . A thin glass cover-slip is positioned as shown at (b) and
pressed firmly onto the shoulders of the chamber; to achieve proper contact it is necessary, while pressing, to move the cover-slip (slightly)
against the shoulders. Proper contact is indicated by the appearance of a pattern of coloured lines (Newtons rings), shown at (b).
Using the chamber. A small volume of a bacterial suspension is picked up in a Pasteur pipette by capillary attraction; the thread of liquid in
the pipette should not be more than 10 mm. The pipette is then placed as shown at (b), i.e., with the opening of the pipette in contact with the
central plateau, and the side of the pipette against the cover-slip. With the pipette in this position, liquid is automatically drawn by capillary
attraction into the space bounded by the cover-slip and one-half of the central plateau; the liquid should not overflow into the trough. (It is
sometimes necessary to tap the pipette, lightly, against the central plateau to encourage the liquid to enter the chamber.) A second sample
can be examined, if required, in the other half of the counting chamber. The chamber is left for 30 min to allow the cells to settle, and counting
is then carried out under a high power of the microscope which is focused on the grid of the chamber. Since the volume between grid and
cover-slip is accurately known, the count of cells per unit volume can be calculated.
A worked example. Each small square in the grid is 1/400 mm2 . As the distance between grid and cover-slip is 1/10 mm, the volume of
liquid over each small square is 1/4000 mm3 , i.e., (for all practical purposes) 1/4,000,000 ml.
Suppose, for example, that on scanning all 400 small squares 500 cells were counted; this would give an average of 500 400(= 1.25) cells
per small square. Thus, since 1.25 cells occur in 1/4,000,000 ml, the sample must contain 1.25 4,000,000 cells per ml, = 5,000,000 cells
per ml.
If the sample was diluted before examination in the counting chamber, the count obtained must be multiplied by the dilution factor: e.g., if
the sample was diluted 1 in 10, the count must be multiplied by 10.
200
cozymase
and expressed in cowpea protoplasts in the absence of RNA2, but requires RNA-2 for encapsidation and for cell-to-cell
spread; expression of RNA-2 is completely dependent on the
expression of RNA-1. Both RNAs appear to be translated (in
the cytoplasm) into large POLYPROTEINS which are cleaved to
form functional proteins. RNA-1 encodes at least 6 proteins,
including VPg and a protease apparently involved in cleavage
of the polyprotein [EMBO (1987) 6 549554]; RNA-2 carries
genes for the capsid proteins. Cells infected with CPMV
contain characteristic inclusion bodies: membranous, vesicular
structures, usually adjacent to the nucleus, which contain
dsRNA corresponding to RNA-1 and RNA-2, complementary
(minus-strand) RNA, and replication complexes containing RNADEPENDENT RNA POLYMERASE molecules. (Although uninfected
cowpea cells contain an RNA-dependent RNA polymerase, the
activity of which increases by 10-fold or more on infection
with CPMV, this enzyme appears not to be involved in CPMV
replication [Book ref. 80, pp. 120125].) Progeny CPMV
particles accumulate in the host cell cytoplasm, sometimes
forming crystalline arrays.
cowpea ringspot virus See CUCUMOVIRUSES.
cowpea severe mosaic virus See COMOVIRUSES.
cowpox A mild disease which primarily affects cows but which is
transmissible (by direct contact) to human handlers; it is caused
by the COWPOX VIRUS. In cows, lesions (which progress from
papules through vesicles and pustules to crusts cf. SMALLPOX)
develop mainly on the udder and teats; other animals (e.g. cats
[VR (1985) 117 231233]) may be affected. In man the lesions
occur mainly on the hands and arms and may be accompanied
by local oedema and lymphangitis.
cowpox virus A virus of the genus ORTHOPOXVIRUS; it is the
causal agent of COWPOX. The virus has a relatively broad host
range, including e.g. cattle, man, and many other animals; it
has been recovered from wild rodents, and rodents may be the
natural reservoir host. Cowpox virus forms large, haemorrhagic
pocks on the CAM, and is highly lethal for chick embryos. Both
A- and B-type inclusion bodies are formed in infected cells.
DNA MWt: ca. 145 106 .
coxibs See PROSTAGLANDINS.
Coxiella A genus of Gram-negative bacteria of the RICKETTSIEAE.
Cells: highly pleomorphic, non-motile rods, ca. 0.20.4
in these cases counts may be given as the number of colonyforming units (cfu) per unit volume or area of the sample; a cfu
can be any entity e.g. a single cell or a chain of cells capable
of giving rise to a single colony.
The above methods are generally applicable e.g. to most
bacteria and spores, and some of the methods may be used for
certain algae, fungi (e.g. yeasts) and protozoa. The counting of
rapidly moving microorganisms can be facilitated by the use
of a viscous suspending medium e.g. FICOLL, methylcellulose
(25% aqueous) or poly(ethylene oxide).
(b) Viruses. Viruses may be counted by electron microscopy,
and the largest viruses (e.g. some entomopoxviruses) may be
counted by light microscopy after suitable staining; however,
such methods are seldom used since e.g. they do not distinguish
between infective and non-infective virions. In the plaque
method of assay, serial dilutions of a viral suspension are initially
prepared, and a known volume of each dilution is examined for
its content of infectious, plaque-forming virions: see PLAQUE (1)
and PLAQUE ASSAY. An alternative procedure is the END-POINT
DILUTION ASSAY. Plant viruses may be assayed on LOCAL LESION
hosts.
coupled cell division See F PLASMID.
coupling sequences See CONJUGATIVE TRANSPOSITION.
cover-glass (cover-slip) A small round or rectangular sheet of
thin glass used primarily to cover a specimen on a microscope
SLIDE. When a slide is viewed with a HIGH-DRY OBJECTIVE lens,
the image quality is optimum only when the cover-glass is of a
particular thickness (specified by the lens manufacturer); thicker
or thinner cover-glasses effectively increase spherical aberration.
Cover-glass thickness is relatively unimportant with low-power
objectives and (usually) with oil-immersion objectives. Coverglasses are made in thickness ranges designated No. 0 (ca.
0.1 mm), No. 1 (ca. 0.15 mm), No. 1 1/2 (ca. 0.175 mm), No.
2 (ca. 0.2 mm), and No. 3 (ca. 0.3 mm). Most objectives
are designed for use with No. 1 1/2 cover-glasses. (See also
CORRECTION COLLAR.)
cover-slip Syn. COVER-GLASS.
covered smut See SMUTS (sense 2).
covirus Syn. MULTICOMPONENT VIRUS.
Cowan I, II & III strains Strains of Staphylococcus aureus used
e.g. for the production of standard TYPING antisera.
Cowdria
A genus of Gram-negative bacteria of the tribe
EHRLICHIEAE. Cells: coccoid to rod-shaped, pleomorphic, nonmotile, maximum dimension ca. 0.5 m. Growth occurs intracytoplasmically in the vascular endothelial cells of ruminants,
but does not occur in cell-free media. Type species (sole
species): C. ruminantium, the causal agent of heartwater (a
tick-borne, septicaemic disease of ruminants which occurs in
Africa); C. ruminantium is transmitted trans-stadially, but not
transovarially, in the tick vector. [Book ref. 22, pp. 709710.]
cowpea aphid-borne mosaic virus See POTYVIRUSES.
cowpea chlorotic mottle virus See BROMOVIRUSES.
cowpea mosaic virus (CPMV) The type member of the COMOVIRUSES. Three types of particle can be distinguished and are
designated T, M and B (S20
w 58, 98 and 118, respectively);
each is icosahedral, ca. 28 nm diam., the capsid consisting of
60 subunits of each of two structural proteins (MWts 22000
and 42000). T particles appear to consist only of protein. B
particles contain a single molecule of RNA-1 (B-RNA, MWt ca.
2 106 ) while the M particles contain one molecule of RNA-2
(M-RNA, MWt ca. 1.2 106 ). Both RNAs are polyadenylated
at the 3 end and have a small polypeptide (VPg, MWt ca.
4000) covalently bound to the 5 end. RNA-1 can be replicated
201
cpd gene
pyridine, quinoline, anthracene and naphthalene. (See also
LENTINUS.)
cross-reacting antibody
schedule, the water in a fixed and washed specimen is initially
replaced by an intermediate fluid (e.g. ethanol or acetone),
and the specimen, totally immersed in the intermediate fluid,
is placed in a strong metal pressure chamber. The chamber is
then closed, cooled to ca. 1518 C, and the intermediate fluid is
replaced by the transitional fluid (usually liquid CO2 ) by means
of a valve system; the specimen remains below the liquidgas
boundary throughout. The liquid CO2 is then partially drained
and fresh liquid CO2 is added; this is repeated several times to
dilute out the intermediate fluid, the specimen always remaining
fully covered by liquid CO2 . When the last traces of intermediate
fluid have been replaced by liquid CO2 the temperature of the
(closed) chamber is slowly raised (e.g. 1 C/ min) above 31 C:
the critical point above which CO2 cannot exist as a liquid.
The gas is then bled off slowly (to avoid e.g. turbulence in the
chamber).
In an alternative schedule, various halocarbons (e.g. certain
Freons) may be used to displace the ethanol or acetone. Thus
e.g. ethanol may be displaced by two different halocarbons,
used sequentially: the first acts as an additional intermediate
fluid, while the second acts as the transitional fluid. (cf. FREEZEDRYING.)
critical temperature zone See FREEZING.
CRM Cross-reacting material: protein which cross-reacts serologically with a given biologically active protein; CRM may
lack the biological activity of the given protein, e.g., it may be
a product of a mutant gene or a precursor form of the given
protein.
cro gene See BACTERIOPHAGE l.
Crohns disease A (typically) chronic human disease of the
intestinal tract which is characterized by granulomatous/ulcerative
lesions; diarrhoea and intestinal pain are common. The acute form
may resemble appendicitis.
The aetiology is not known. Possibly, mutations affecting
certain intracellular molecules in the intestinal epithelium (e.g.
Nod2) may affect the normal protective response to bacterial
infection [JBC (2003) 278 55095512, 88698872].
cromoglycate A therapeutic agent which stabilizes sensitized
MAST CELLS, inhibiting the release of histamine; it is administered
before the patient is exposed to antigen/allergen in order to
prevent anaphylactic reactions.
Cronartium
A genus of rust fungi (class UREDINIOMYCETES)
which include some important parasites of pine trees (Pinus
spp): see e.g. BLISTER RUST. (See also PERIDERMIOID.)
cross-feeding (1) Syn. SYNTROPHISM. (2) A particular type of
SYNTROPHISM in which each organism derives essential growth
factors from the other(s).
cross-linking quantitative assay A type of assay which has been
used for detecting and quantifying hepatitis B virus (HBV) in
serum. The assay, carried out in the solution phase, involves
probes which incorporate a derivative of 7-hydroxycoumarin a
cross-linking agent that can be photo-activated by ultraviolet
radiation such that each probe can be covalently bound to its
target sequence in HBV DNA. Essentially, probes complementary to sequences in the major subtypes of HBV are allowed
to hybridize to target sequences in the sample and are then
photo-cross-linked to their targets; by means of biotin tags, the
cross-linked probes are captured on streptavidin-coated DYNABEADS and subsequently labelled with alkaline phosphatase.
The addition of a suitable substrate for the enzyme gives rise to
a fluorescent signal. [Cross-linking assay for HBV DNA: JCM
(1999) 37 161164.]
cross-reacting antibody Antibody which can combine with nonhomologous antigen (i.e. antigen not identical to that which
203
cross-reacting material
elicited the antibody) as well as with homologous antigen.
Such cross-reaction requires that the homologous and nonhomologous antigens have a certain degree of stereochemical
similarity. Cross-reacting antibodies often have a much lower
affinity for the non-homologous antigen (cf. HETEROCLICITY.)
(See also MONOCLONAL ANTIBODIES.)
Antibodies raised against a particular microorganism may
combine with related (or even unrelated) species (see e.g.
WEILFELIX TEST); such organisms may share a common antigenic determinant or may have CROSS-REACTIVE ANTIGENS.
cross-reacting material See CRM.
cross-reactivation See REACTIVATION.
cross-reactive antigens Antigens which differ from one another
but which can combine with antibodies raised against either (or
any) one of them. In type 1 cross-reactivity, different crossreactive ligands bind with different affinities to a given site
on a given antibody molecule; in type 2 cross-reactivity a
cross-reactive ligand reacts with some of the antibodies in a
POLYCLONAL ANTISERUM raised against the homologous ligand
[Mol. Immunol. (1981) 18 751763].
cross resistance The phenomenon in which the resistance of an
organism to one antibiotic correlates with resistance to one or
more other antibiotics.
cross-wall Syn. SEPTUM.
crossband (in prosthecae) See CAULOBACTER.
crossed immunoelectrophoresis See TWO-DIMENSIONAL ELECTROPHORESIS.
crossing over A RECOMBINATION process in which, e.g., exchange
of double-stranded sequences occurs between two linear
duplexes. In effect, crossing over involves a break in each of
the two strands in both (linear) duplexes, exchange of parts of
the duplexes, and ligation to form two recombinant duplexes (see
RECOMBINATION). Thus, if the two duplexes carry alleles ABCD
and abcd, crossing over results in recombinant molecules Abcd
and aBCD, ABcd and abCD, or ABCd and abcD, depending on
the site of the cross-over. In e.g. MEIOSIS, crossing over occurs
between non-sister chromatids in homologous chromosomes (cf.
PARASEXUAL PROCESSES).
If crossing over occurs between two circular molecules the
result is a single larger circular molecule; conversely, crossing
over between regions within a single circular molecule results
in two smaller circular molecules. (See also CAMPBELL MODEL.)
crotocin See TRICHOTHECENES.
croup A type of laryngotracheitis with hoarseness, resonant
cough, stridor, and respiratory obstruction. Croup occurs mainly
in young children and may be of non-microbial causation (e.g.
allergy) or due to infection by e.g. human respiratory syncytial
virus, parainfluenza viruses, Corynebacterium diphtheriae.
crown gall A plant neoplasm, sometimes bearing root-like,
stem-like and/or leaf-like structures, which is formed at the
crown (stemroot junction) or, less commonly, on stems or
roots in a wide range of gymnosperms and dicotyledonous
angiosperms (although in few monocotyledonous angiosperms);
crown gall follows infection of a wound with virulent strains
of certain species of Agrobacterium, commonly A. tumefaciens
(see AGROBACTERIUM). Infected plants may be stunted or even
killed; the disease can cause important economic losses (for
example, in stone-fruit trees and vines) e.g. in parts of Australia,
Europe and the USA. Crown gall of grape is caused by strains
of Agrobacterium which have been assigned to a new species,
A. vitis [crown gall of grape (biology and disease management):
ARPpath. (1999) 37 5380]. (See also GALLS.)
A. tumefaciens attaches to the host plant at the site of a
wound, attachment being reported to occur via the bacterial
Cryptococcus
+
cryosubstitution FREEZE-SUBSTITUTION.
cryotome See FREEZE-SECTIONING.
Cryoxicide A STERILANT containing ETHYLENE OXIDE (11%),
trichlorofluoromethane (79%), and dichlorodifluoromethane
(10%).
crypt (ciliate protozool.) See BROOD POUCH.
cryptic mutant A cell which lacks one or more components of
a TRANSPORT SYSTEM so that a particular substrate, or substrates,
cannot enter the cell and hence cannot be utilized, even though
the cell may possess all the enzymes necessary for its utilization.
For example, the failure of a cell to produce enzyme I (see
PTS) as a result of a (pleiotropic) mutation would prevent
that cell (a cryptic mutant) from taking up and metabolizing a
range of sugars.
cryptic plasmid A PLASMID which has no apparent effect on the
phenotype of the cell in which it occurs.
cryptic viruses Virus-like isometric particles which have been
detected in a wide range of symptomless plants; the particles
are generally ca. 30 nm in diameter, are present in low concentrations, and appear to be seed-borne. Some have been shown
to contain dsRNA [e.g. beet cryptic viruses: JGV (1986) 67
363366].
cryptidin See DEFENSINS.
Cryptobia See BODONINA.
cryptobiosis See DORMANCY.
Cryptocaryon
A genus of cyst-forming ciliates related to
ICHTHYOPHTHIRIUS; the sole species, C. irritans, causes WHITE
SPOT in marine fish.
Cryptococcaceae A family of fungi of the class BLASTOMYCETES. The genera include CANDIDA, CRYPTOCOCCUS, KLOECKERA, RHODOTORULA and TRICHOSPORON.
cryptococcosis (torulosis; also European blastomycosis or Busse
Buschke disease) A disease of man and animals caused
by Cryptococcus neoformans (q.v.); infection occurs on
inhalation of dust contaminated with the fungus. Pulmonary
infection may be mild or inapparent. However, particularly in
individuals with e.g. defective CMI or certain leukaemias, the
disease may become disseminated to almost any tissue (liver,
bones, skin etc) but especially to the meninges (cryptococcal
MENINGITIS commonly fatal). Diagnosis: demonstration of
the fungus by culture or microscopy; latex particle test
for cryptococcal capsular polysaccharide. Chemotherapy:
e.g. amphotericin B, flucytosine, possibly miconazole or
ketoconazole. [Book ref. 17, pp. 180186.]
Cryptococcus
A genus of non-fermentative imperfect yeasts
(class HYPHOMYCETES). The cells are spheroidal, ovoid, elongate,
or polymorphic, and reproduce by multilateral budding.
Pseudomycelium is rudimentary or absent. The vegetative
cells usually have capsules, the composition of the capsule
and the abundance of capsular material depending on growth
conditions; under certain conditions the capsule contains starchlike polysaccharides which may be released into the medium.
Colonies on e.g. malt agar are typically mucoid and are
commonly cream- to tan-coloured, or red in some species (e.g.
C. hungaricus and C. macerans). Inositol can be assimilated as
sole carbon source. NO3 is assimilated by some species.
Most Cryptococcus species have basidiomycetous affinities:
C. albidus var. albidus and C. uniguttulatus are anamorphs
of FILOBASIDIUM spp, C. neoformans of FILOBASIDIELLA sp.
Three species have ascomycetous affinities: C. cereanus and
C. lactativorus, which are anamorphs of SPOROPACHYDERMIA,
and C. melibiosum (teleomorph unknown). [Book ref. 100, pp.
845872.]
cryptoendolith
C. neoformans is the causal agent of CRYPTOCOCCOSIS and
may also be associated with e.g. bovine mastitis. Cells (e.g. in
malt extract after 3 days at 25 C) are spherical, ca. 38 m
diam., occurring singly, in pairs, or in small groups. Pseudomycelium is not formed, and extracellular polysaccharide may
be abundant. C. neoformans is the only Cryptococcus sp which
can grow well at 37 C (certain other species or strains e.g.
C. melibiosum may be capable of weak growth at 37 C).
C. neoformans has two varieties, var. neoformans and var. gattii (= C. bacillisporus), distinguished e.g. on the basis of the
ability of var. gattii (but not var. neoformans) to give a blue
colour on CGB AGAR within 25 days.
Other Cryptococcus spp (not mentioned above) include
e.g. C. ater, C. dimennae, C. elinovii, C. flavus, C. gastricus,
C. heveanensis, C. infirmo-miniatus, C. kuetzingii, C. laurentii,
C. luteolus, C. magnus, C. skinneri, C. terreus. Strains have
been isolated from a wide range of habitats, including e.g. soil,
plants, dew-retted flax, seawater, clinical specimens, foods and
beverages, etc. Another species, C. friedmannii, has been isolated from rock fragments containing cryptoendolithic lichens
from a dry desert area of the Antarctic [Mycol. (1985) 77
149153].
cryptoendolith See ENDOLITHIC.
cryptogam A plant which does not produce true flowers or seeds;
cryptogams traditionally include the ALGAE, FUNGI, bryophytes
(e.g. mosses) and pteridophytes (e.g. ferns).
cryptogram (virol.) A descriptive code used to summarize, in
symbolic form, certain basic properties of a given virus.
Cryptomonadida See PHYTOMASTIGOPHOREA.
cryptomonads Syn. CRYPTOPHYTES.
Cryptomonas See CRYPTOPHYTES.
cryptophytes (cryptomonads) A category of unicellular, biflagellated, marine or freshwater organisms variously regarded
as algae (class Cryptophyceae) or as protozoa (see PHYTOMASTIGOPHOREA); most cryptophytes are photosynthetic
(including e.g. Chroomonas and Cryptomonas), but some (e.g.
Chilomonas, Cyathomonas) are colourless and heterotrophic.
The cryptophyte cell is typically flattened and dorsiventral, lacks
a cell wall (having instead a plasma membrane with an internal
lining of proteinaceous plates), and possesses EJECTOSOMES. In
photosynthetic species each cell has a single bilobed chloroplast
containing a pyrenoid, paired thylakoids, chlorophylls a and c2 ,
a-carotene, diatoxanthin, and PHYCOBILIPROTEINS. Storage products are starch and lipid. Reproduction occurs by longitudinal
binary fission; sexual reproduction is unknown. [Taxonomic
aspects (including genus descriptions): New Phyt. (1984) 98
627646.]
cryptosporidiosis A COCCIDIOSIS (q.v.) of man and other animals
caused by a species of CRYPTOSPORIDIUM; the pathogen is
commonly transmitted (as sporulated oocysts) via the direct or
indirect faecaloral route.
The disease in man is typically mild and self-limiting; it
may involve diarrhoea, abdominal cramps, low-grade fever and
headache. In the severely immunocompromised it is a lifethreatening disease: usually severe, persistent watery diarrhoea;
other sites (e.g. respiratory, biliary) may be affected. No effective
chemotherapy is available [IJP (1995) 25 139195]. [The
treatment dilemma: JMM (2000) 49 207208.]
Cryptosporidium is a cause of diarrhoea, pneumonia and
disseminated infections in calves foals, lambs and piglets; it
can also cause diarrhoea, inappetance and weight loss in the
domestic cat [VR (1985) 116 7374].
[Cryptosporidiosis in animals and humans: MR (1983) 47
8496.]
Outbreaks of disease can be transmitted via water as thickwalled oocysts of Cryptosporidium are resistant to the level
of chlorination normally used in WATER SUPPLIES. The viability
of C. parvum oocysts in water has been examined by staining
them with fluorescent dyes (SYTO-9, SYTO-59); oocysts which
stained above a certain intensity could not establish infection in
mice, but those which displayed little or no fluorescence could
readily establish infection [AEM (2000) 66 406412].
Cryptosporidium A genus of parasitic (homoxenous) protozoa
(suborder EIMERIORINA q.v.) which are pathogenic for man and
other animals (see CRYPTOSPORIDIOSIS); the organisms typically
develop in the intestinal microvilli. The oocysts are very small
(ca. 46 m); following ENDOSPORULATION, each oocyst contains
four banana-shaped sporozoites. Two types of oocyst are formed;
thin-walled oocysts which release sporozoites into the hosts
intestine, causing re-infection (autoinfection) of the host, and
acid-fast thick-walled oocysts (ca. 80% of the total) which are
voided in the faeces.
[Complete development of Cryptosporidium in cell cultures:
Science (1984) 224 603605.]
The taxonomy of the genus is unsettled. It has been suggested
that only 4 species should be recognized e.g. on the basis of host
range: C. crotali (infecting reptiles), C. meleagridis (infecting
birds), C. muris (infecting mammals) and C. nasorum (infecting
tropical fish) [JP (1984) 31 9498]. However, C. parvum,
the organism which appears to be the cause of most cases
of cryptosporidiosis, is apparently distinct from C. muris [J.
Parasitol. (1985) 71 625629]. [C. baileyi from chickens: JP
(1986) 33 289296.]
Cryptostroma See HYPHOMYCETES; see also MAPLE BARK STRIPPERS DISEASE and SOOTY BARK.
crystal toxin (of Bacillus thuringiensis) See DELTA-ENDOTOXIN.
crystal violet A violet basic TRIPHENYLMETHANE DYE used e.g. in
the GRAM STAIN.
CS protein See PLASMODIUM.
CS1, CS2, CS3 See ETEC.
CSF (1) Cerebrospinal fluid. (2) COLONY-STIMULATING FACTOR.
(3) Cold stability factor (see MICROTUBULE-ASSOCIATED PROTEINS). (4) A pheromone of Bacillus subtilis (see QUORUM SENSING).
CSLM CONFOCAL SCANNING LIGHT MICROSCOPY.
CSP reaction Shedding of CS proteins by the sporozoites of
Plasmodium spp (see PLASMODIUM) following cross-linking of
the CS proteins by anti-CS antibodies. (cf. Capping phenomenon
in DYSENTERY (b).)
CspA See COLD-SHOCK RESPONSE.
CSPD Trade name (Tropix, Bedford, MA, USA) of a 1,2dioxetane substrate which gives rise to CHEMILUMINESCENCE
when activated by the enzyme alkaline phosphatase. (See also
AMPPD.)
CSSD Central sterile supply department.
CTAB See QUATERNARY AMMONIUM COMPOUNDS.
ctDNA Chloroplast DNA (see CHLOROPLAST).
CTEM Conventional transmission ELECTRON MICROSCOPY.
CTh CARRIER-SPECIFIC T HELPER CELL.
CTLA-4 See CD28.
CTP Cytidine 5 -triphosphate [see Appendix V(b)].
ctxA, ctxB genes See CHOLERA TOXIN.
cucumber 4 virus See TOBAMOVIRUSES.
cucumber green mottle mosaic virus See TOBAMOVIRUSES.
cucumber mosaic virus See CUCUMOVIRUSES.
cucumber necrosis virus See TOBACCO NECROSIS VIRUS.
cucumber pale fruit viroid See VIROID.
206
curdlan
cucumbers (pickled) See PICKLING.
cucumoviruses (cucumber mosaic virus group) A category of
ssRNA-containing PLANT VIRUSES which infect e.g. cucurbits
and solanaceous plants; transmission occurs (non-persistently)
via aphids and, in some hosts, via seeds, and can also occur
mechanically. Type member: cucumber mosaic virus, CMV (S
isolate). Other members: peanut stunt virus (PSV) and tomato
aspermy virus (TAV); possible member: cowpea ringspot virus.
Virion: icosahedral, ca. 29 nm diam., containing a single
type of coat protein and linear, positive-sense ssRNA. Three
types of virion exist, differing in the nature of the RNA they
contain; a particle may contain one molecule of RNA-1 (MWt
ca. 1.27 106 ), one molecule of RNA-2 (MWt ca. 1.13 106 ),
or one molecule each of RNA-3 (MWt ca. 0.82 106 ) and
RNA-4 (coat protein mRNA). Some isolates of CMV and PSV
also contain SATELLITE RNAS designated (respectively) CARNA
(CMV-associated RNA) and PARNA (P SV-associated RNA).
CARNA 5, the best-known example, consists of 335 nucleotides
and is capped at the 5 end; it can code for two polypeptides.
The presence of a CARNA attenuates the symptoms of CMV
infection in many plants, but may enhance disease severity
in others. For example, in tomato plants infection with CMV
(only) may cause leaf chlorosis with some leaf distortion, but
infection with both CMV and CARNA 5 causes a lethal necrosis.
White leaf of tomatoes and brilliant yellowing of tobacco
are also examples of diseases caused by CARNA strains. The
presence of a CARNA in a host plant also reduces the yield of
CMV apparently as a result of competition for virus replication
machinery.
Cucurbitaria See DOTHIDEALES.
cud See RUMEN.
cudbear A purple dye obtained from Ochrolechia tartarea.
Culex A genus of mosquitoes (order Diptera, family Culicidae);
Culex spp are vectors of certain diseases: see e.g. MURRAY
VALLEY FEVER.
Culicinomyces
A genus of fungi of the HYPHOMYCETES;
C. clavisporus is pathogenic in mosquito larvae [Mycol. (1984)
76 614625].
Culicoides
A genus of biting midges (order Diptera, family
Ceratopogonidae); Culicoides spp are vectors of certain diseases:
e.g. AFRICAN HORSE SICKNESS and BLUETONGUE.
culmination See DICTYOSTELIOMYCETES.
cultivar (cv.) A commercial or cultivated variety of a given
species of plant or fungus.
culture (1) (noun) A liquid or solid MEDIUM on or within which
has grown a population of particular type(s) of microorganism
or cell as a result of the prior INOCULATION and INCUBATION
of that medium. The following refers primarily to microbial
cultures cf. TISSUE CULTURE. On a solid medium, microorganisms may grow as a continuous layer or film of surface
growth (confluent growth) or as discrete (individual) colonies
(see COLONY) depending e.g. on the method of inoculation (cf.
LAWN PLATE and STREAKING). Cultures in liquid media may be
turbid or clear, and may or may not have a PELLICLE.
Aerobic culture. A culture prepared under AEROBIC (sense 1)
conditions.
Anaerobic culture. One prepared under ANAEROBIC (sense 1)
conditions. (See also ANAEROBE.)
Axenic culture. Pure culture (see below).
Batch culture. See BATCH CULTURE.
Broth culture. One prepared with NUTRIENT BROTH or with any
similar liquid medium.
Closed culture. Syn. BATCH CULTURE.
Contaminated culture. One which has been exposed (usually unintentionally) to non-STERILE conditions and which has
become contaminated with extraneous organisms.
Continuous culture. See CONTINUOUS CULTURE.
Fed batch culture. See FED BATCH CULTURE.
Mixed culture. One containing two or more species or strains
of organism.
Old culture. One which has been incubated or stored for
an excessive period of time and in which, as a consequence,
degenerative changes may have occurred see e.g. INVOLUTION
FORMS.
Open culture. Syn. CONTINUOUS CULTURE.
Plate culture (plate). One prepared using a solid medium
(e.g. nutrient agar) in a PETRI DISH.
Primary culture. See PRIMARY CULTURE.
Pure culture (AXENIC culture). One in which all the organisms
are of the same species or strain.
Shake culture. See SHAKE CULTURE.
Slant culture. Slope culture (see below).
Slope culture (slant culture). One prepared using a SLOPE.
Stab culture. One produced by deep inoculation of a solid
medium (e.g. the butt of an agar or gelatin slope) with a STRAIGHT
WIRE; the wire is pushed vertically into the medium so that the
INOCULUM (on the tip of the wire) is distributed along the length
of the stab.
Subculture. See SUBCULTURE.
Synchronous culture. See SYNCHRONOUS CULTURE.
(2) (noun) The process of preparing a culture (sense 1).
(3) (verb) To encourage the growth of particular type(s) of
microorganism under controlled conditions. Cultures of bacteria
or fungi are usually started by seeding (inoculating) a medium
with viable cells or spores from another culture, or by inoculating the medium with material expected to contain particular
type(s) of viable organism; the type of MEDIUM and the incubation conditions required differ widely among the different types
of microorganism. Certain organisms (e.g. Rickettsia spp, Treponema pallidum) can be cultured only in living systems. (See
also ASEPTIC TECHNIQUE; ENRICHMENT; LOOP.)
culture collections Collections of characterized microorganisms.
General collections: see e.g. ATCC, CBS, CCM, CIP, DSM, JCM, LMD,
and NCTC; agricultural (including dairy and phytopathological
organisms): see e.g. ICPB, NCDO, NCPPB, NRRL and UWO; algae: see
e.g. SAG; fungi (including yeasts): see e.g. CBS and CMI; industrial
and applied; see e.g. IAM, IFO and NCIB; marine bacteria; NCMB;
medical : see e.g. CDC.
cultured (of bacteria etc.) Grown.
cultured butter See BUTTER.
cultured buttermilk See BUTTERMILK.
Cummings disease See AVIAN INFECTIOUS BRONCHITIS.
Cunninghamella See MUCORALES.
Cunninghamellaceae See MUCORALES.
cup fungi Ascomycetes which form cup-like fruiting bodies,
particularly members of the PEZIZALES.
cup lichens Species of CLADONIA whose podetia have conspicuous scyphi.
cuprammonium hydroxide See COPPER.
cupredoxin See BLUE PROTEINS.
cupulate Cup-Shaped. (See also AECIDIOID.)
curdlan A class of extracellular, water-insoluble, linear (1 3)b-glucans formed e.g. by Alcaligenes faecalis var. myxogenes
and by strains of Agrobacterium and Rhizobium. When aqueous
suspensions of curdlans (e.g. 2% w/v) are heated to >90 C
and then cooled slowly, they form very elastic, resilient gels.
207
curie
cut-and-paste mechanism (of transposition) See e.g. Tn10.
cutaneous basophil hypersensitivity Syn. JONESMOTE SENSITIVITY.
cutaneous herpes See HERPES SIMPLEX.
cutaneous leishmaniasis LEISHMANIASIS of man and other animals in which the pathogen primarily infects the skin and gives
rise to self-healing or metastasizing lesions; the causal agents
(which are transmitted by sandflies), and the patterns of disease,
vary with geographical location.
Old World cutaneous leishmaniases (mainly in Africa and
Asia) are typically caused by Leishmania aethiopica, L. major
or L. tropica. In man, a papule develops (after several weeks)
at the site of a sandfly bite, becoming necrotic at the centre and forming a moist, ulcerative lesion (L. major) or a dry
lesion (L. aethiopica, L. tropica) which eventually heals. (These
lesions have been called e.g. Aleppo boil, Delhi boil, oriental
sore.) L. aethiopica and L. major infections are zoonotic, animal reservoirs including populations of e.g. the great gerbil,
Rhombomys opimus (for L. major), and the rock hyrax, Procavia capensis (for L. aethiopica); L. tropica infections appear
to be anthroponotic.
New World cutaneous leishmaniases (in South America) are
caused by L. braziliensis or L. mexicana; they are zoonotic
diseases in man, animal reservoirs including rodents and sloths.
The clinical picture in man may resemble the Old World pattern;
however, following an apparent cure the disease may re-appear
at a site remote from the original lesion, and in some cases the
infection may metastasize to the oral/nasal mucous membranes
(see MUCOCUTANEOUS LEISHMANIASIS).
(See also CHICLEROS EAR and PIAN BOIS.)
Diagnosis of cutaneous leishmaniasis may involve e.g. microscopical examination of exudate from lesions, culture of lesion
material (in e.g. NNN MEDIUM), and the MONTENEGRO TEST; treatment may involve e.g. pentavalent ANTIMONY compounds and/or
antibiotics.
(cf. VISCERAL LEISHMANIASIS.)
cutaneous T-cell lymphoma See MYCOSIS FUNGOIDES and SEZARY
SYNDROME; see also ADULT T-CELL LEUKAEMIA.
cuticle (mycol.) Syn. PELLIS.
cutin An insoluble polymer which, embedded in waxes, forms
the cuticle which covers the epidermal cell walls in the aerial
parts of higher plants. (cf. SUBERIN.) Cutin is a polyester
formed from C16 and C18 hydroxy fatty acids. It functions
as a physical barrier, protecting against water loss, entry of
pathogens, etc. Many plant-pathogenic fungi produce enzymes
(cutinases) which can breach the cutin barrier prior to infection.
[Book ref. 58, pp. 79100; enzymic penetration of the plant
cuticle by fungal pathogens: ARPpath. (1985) 23 223250.]
cutinase A CUTIN-degrading enzyme.
cutis (mycol.) Syn. PELLIS.
Cutleria See PHAEOPHYTA.
cv. CULTIVAR.
CVF COBRA VENOM FACTOR.
Cx cellulase See CELLULASES.
CY agar A medium which includes pancreatic digest of casein,
yeast autolysate, and (sometimes) CaCl2 .
cya gene See ADENYLATE CYCLASE.
cyaA gene See CYCLOLYSIN.
cyanelles Endosymbiotic CYANOBACTERIA which occur in various
eukaryotes: e.g. in the testate amoeba PAULINELLA, in the algae
Cyanophora paradoxa and Glaucocystis spp, and in certain
sponges; many contain CARBOXYSOMES. A number of authors
consider that cyanelles were the evolutionary precursors of
CHLOROPLASTS. (See also GLAUCOPHYTA.)
cyanobacteria
can also catabolize endogenous polysaccharide under anaerobic conditions either by anaerobic respiration using sulphur as
terminal electron acceptor (resulting in sulphide formation) or
by a fermentative pathway in which lactic acid is produced.
Some cyanobacteria can grow on exogenous organic compounds either photoheterotrophically or chemoorganotrophically. [Carbon metabolism: Ann. Mic. (1983) 134 B 93113.]
Certain species (e.g. Cyanothece halophytica, Dactylococcopsis salina, Oscillatoria limnetica) can, in the presence of sulphide, carry out facultative anoxygenic PHOTOSYNTHESIS using
photosystem I with H2 S as electron donor; in O. limnetica the
resulting sulphur accumulates extracellularly. NITROGEN FIXATION
occurs in many species, usually in specialized cells called HETEROCYSTS (cf. GLOEOTHECE and TRICHODESMIUM): see also NIFGENES. In some species (e.g. Anabaena variabilis) diazotrophy
can occur in the dark under heterotrophic conditions [energy
requirement: JGM (1983) 129 26332640]. [General metabolic
aspects: Book ref. 76.]
Cyanobacteria occur in a wide range of habitats, from tropical
to polar regions; however, they are rare or absent in habitats of
pH < ca. 5. Depending on species, they may be found in fresh,
brackish, marine and hypersaline waters, where they may be
planktonic, benthic, epiphytic etc (see also BLOOM and OSMOREGULATION); in hot springs; on soils (including hot arid desert
soils), muds, sediments and salt-marshes (where they may form
extensive and conspicuous mats); on rocks (where they may be
endolithic or epilithic); etc. (See also STROMATOLITE.) In many
such environments (including rice fields) free-living cyanobacteria may be important providers of fixed nitrogen, and certain
nitrogen-fixing cyanobacteria form symbiotic associations with
eukaryotic organisms (see e.g. ANABAENA and NOSTOC). Heterocystous cyanobacteria of several genera (Anabaena, Cylindrospermum, Gloeotrichia, Nostoc) occur in colonies attached
to the lower epidermis or in the reproductive pockets in the
leaves of floating duckweed plants (Lemnaceae), possibly supplying much of their nitrogen requirement [CJM (1985) 31
327330]. (See also CYANELLE; RHIZOSOLENIA; RHOPALODIA.) No
species appears to be directly pathogenic in any organism,
but some freshwater bloom-forming strains produce potent toxins which may cause illness or death in animals drinking the
water (see e.g. ANABAENA, APHANIZOMENON, MICROCYSTIS, NODULARIA; cf. LYNGBYA), and cyanobacterial blooms in reservoirs
may cause tainting of the WATER SUPPLIES (see e.g. GEOSMIN).
[Toxins and health: RMM (1994) 5 256264.] Cyanobacterial
toxins (= cyanotoxins) include e.g. (i) neurotoxins such as the
anatoxins (see ANABAENA) and SAXITOXIN; (ii) hepatotoxins such
as microcystins (produced by strains of MICROCYSTIS and of e.g.
Anabaena, Nostoc and Oscillatoria); (iii) dermatotoxins such as
aplysiatoxin (produced by strains of LYNGBYA and of e.g. Oscillatoria). [Ecological and molecular investigations of cyanotoxin
production (review): FEMS Ecol. (2001) 35 19.]
Fossil organisms resembling cyanobacteria are among the
oldest fossils known; from the fossil record and other data it
is believed that cyanobacteria may have dominated the Earths
biota during the middle to late Precambrian (Proterozoic, ca.
2500570 million years ago), and were probably responsible
for the generation of oxygen in the atmosphere. [Book ref. 76,
pp. 543564.]
The taxonomy of the cyanobacteria is confused. Until quite
recently they were regarded as algae and were therefore subject to the Botanical Code of nomenclature. Thus, herbarium
specimens, or descriptions and illustrations, were used as type
materials (living cultures not being recognized as valid types
Cyanobacteriales
Many genera have yet to be incorporated in this scheme:
see e.g. APHANIZOMENON, COELOSPHAERIUM, DACTYLOCOCCOPSIS,
MICROCYSTIS, STARRIA, TRICHODESMIUM.
[Isolation, media etc: Book ref. 45, pp. 212246.]
Cyanobacteriales An order proposed for the CYANOBACTERIA
[IJSB (1978) 28 16] but not accepted as legitimate owing
to the lack of a genus named Cyanobacterium; however, the
proposal of a new genus Cyanobacterium [Ann. Mic. (1983)
134 B 2136] paves the way for legitimization of the order.
Cyanobacterium See SYNECHOCOCCUS and CYANOBACTERIALES.
cyanobiont A cyanobacterial symbiont: see e.g. ANABAENA and
NOSTOC. (cf. PHYCOBIONT.)
Cyanobium See SYNECHOCOCCUS.
cyanocobalamin See VITAMIN B12 .
Cyanocyta See GLAUCOPHYTA.
cyanogen bromide (CNBr) A reagent used e.g. for the IMMOBILIZATION of a protein on the surface of a support; CNBr binds
to the support (forming a CNBr-activated support) and then
binds spontaneously to primary amino groups on the protein.
The instability of the isourea bond (between the activated support and protein) may lead to some loss of the immobilized
protein; this may be avoided e.g. by cross-linking the protein
with glutaraldehyde.
cyanogenic Having the capacity to produce cyanide (see also
CYANIDE sense 2).
cyanoguanidine Dicyandiamide, a NITRIFICATION INHIBITOR.
cyanomycin An antibiotic produced by Streptomyces cyanoflavus and reported to be identical to PYOCYANIN [J. Antibiot.
(1969) 22 4954 cited in JB (1980) 141 156163].
cyanophage Any VIRUS whose host is a cyanobacterium (bluegreen alga). (cf. PHYCOVIRUS.) Cyanophages may be virulent
or temperate, and have been isolated from filamentous and
unicellular species including members of the LPP group
(cyanophages LPP-1, LPP-2), Nostoc (N1, N2), and Anabaena
(A1, A2); lysis of infected intercalary cells in filamentous species
results in progressive fragmentation of the filament. [Ann. Mic.
(1983) 134 B 4359; classification and nomenclature: Intervirol.
(1983) 19 6166.]
cyanophilic Having an affinity for blue dyes such as LACTOPHENOL COTTON BLUE.
Cyanophora See GLAUCOPHYTA.
cyanophycean starch A glycogen-like storage polysaccharide
found in cyanobacteria; the polysaccharide occurs as granules
or rods located between the thylakoids.
cyanophycin (multi-L-arginyl-poly(L-aspartic acid); arg-poly(asp))
A high-MWt polymer consisting of equal amounts of L-aspartic
acid and L-arginine; the L-aspartic acid residues occur in a linear
chain, and each residue is linked via its free carboxyl group to the
a-amino group of an arginine residue. Granules of cyanophycin
(a granules, structured granules) occur in most cyanobacteria.
The polymer is synthesized independently of ribosomes and
serves primarily as a nitrogen reserve in both vegetative cells
and heterocysts. Under CO2 -limiting conditions, cyanophycin
may also serve as a source of carbon and energy by an ARGININE
DIHYDROLASE pathway, at least in some species. [Review: ARM
(1984) 38 1316.]
cyanophytes CYANOBACTERIA.
cyanosis (med., vet.) A bluish discoloration or darkening of the
skin and mucous membranes due to inadequate oxygenation of
the blood.
cyanosomes Cyanobacterial PHYCOBILISOMES.
Cyanothece See SYNECHOCOCCUS.
cyanotoxin Any toxin produced by a member of the CYANOBACTERIA (q.v. for examples).
cyclolysin
more essential stages of its life cycle in the vector. (See e.g.
and TRYPANOSOMA.)
Cyclidium A genus of ciliates (order SCUTICOCILIATIDA) which
occur e.g. in soil, fresh water (including hot springs) and
marine habitats. Cells: typically ovoid and generally small, ca.
1540 m; the cell surface is typically not densely ciliated, but
those cilia which are present tend to be long, and there is often
one or more longer caudal cilia.
cyclin A type of protein involved in the regulation of the
eukaryotic CELL CYCLE. During the cycle, molecules of cyclin
accumulate intracellularly at specific stages and form complexes
with certain PROTEIN KINASES. Phosphorylation of the kinase part
of the complex and subsequent (partial) dephosphorylation at
an appropriate point in the cycle leads to activation of the
kinase. The activated kinase phosphorylates certain proteins
which then promote onward cycling; it can also bring about
UBIQUITIN-dependent degradation of the cyclin so that the
intracellular concentration of cyclin falls sharply on passage
through the checkpoint.
There are various types of cyclin, and different types may
form complexes with protein kinases at different cell-cycle
checkpoints; for example, different types of cyclin form complexes with the yeast protein kinase Cdc2 in order to mediate
passage through (a) the start checkpoint, and (b) the G2 M
checkpoint.
cyclitol antibiotics ANTIBIOTICS which contain a cyclic alcohol e.g. AMINOGLYCOSIDE ANTIBIOTICS (which contain a substituted INOSITOL).
cycloalkanes See HYDROCARBONS.
cycloamyloses Syn. SCHARDINGER DEXTRINS.
cyclochlorotine Syn. CHLOROPEPTIDE.
cyclodextrins Syn. SCHARDINGER DEXTRINS.
cycloguanil See CHLORGUANIDE.
cyclohexane metabolism See HYDROCARBONS.
cycloheximide (Actidione; b-[2-(3,5-dimethyl-2-oxocyclohexyl)2-hydroxyethyl]-glutarimide) An ANTIBIOTIC produced by
certain strains of e.g. Streptomyces griseus; it is a by-product
of streptomycin manufacture. Cycloheximide is active against
many fungi and other eukaryotes (bacteria are not affected),
acting primarily by inhibiting PROTEIN SYNTHESIS; e.g., it
prevents translocation by binding to the 60S subunit of 80S
ribosomes. Ribosomes from different organisms may differ in
sensitivity. Only the yeast-like forms of certain dimorphic fungi
(e.g. Blastomyces dermatitidis, Histoplasma capsulatum) are
susceptible to cycloheximide.
Certain stereoisomers of cycloheximide (e.g. naramycin B)
have been isolated from Streptomyces cultures; these are generally less active than cycloheximide against fungi. Streptovitacins are monohydroxyl-substituted cycloheximides produced
by S. griseus; streptovitacin A appears to resemble cycloheximide in its mode of action.
cyclolysin An RTX TOXIN produced by species of Bordetella. The
177 kDa protein is encoded by gene cyaA; activity of the toxin
depends on post-translational modification in which a long-chain
fatty acid is linked covalently at a specific lysine residue. The
toxin is secreted by an ABC EXPORTER.
Cyclolysin has ADENYLATE CYCLASE, haemolysin and poreforming activity. A range of eukaryotic cells are susceptible;
within the target cell cyclolysin is activated by CALMODULIN.
The principal role of cyclolysin in WHOOPING COUGH may
involve inhibition of the activity of phagocytic cells (e.g.
macrophages) by raising their intracellular levels of cAMP.
Moreover, by suppressing anti-bacterial activity in phagocytes,
PLASMODIUM
adenine
5
CH2 O
HO
O
H
2
OH
cyclo-oxygenase
cyprofuram See PHENYLAMIDE ANTIFUNGAL AGENTS.
Cyrtophorida See HYPOSTOMATIA.
cyrtos (cytopharyngeal basket; nasse; pharyngeal basket) A (frequently curved) type of CYTOPHARYNGEAL APPARATUS whose
walls are strengthened by longitudinal nematodesmata (which
arise at apical kinetosomes) and are lined with extensions of
POSTCILIARY MICROTUBULES; toxicysts are absent. The cyrtos is
characteristic of the HYPOSTOMATIA. (cf. RHABDOS.)
cyst A specialized microbial cell produced either in response to
adverse environmental conditions or as a normal part of the
life cycle. During cyst formation (encystment), an organism
produces a thick or thin wall within which it becomes totally
enclosed. Cysts are usually resistant to desiccation, and may be
resistant to e.g. ultraviolet radiation and/or heat.
(a) (bacteriol.) Cyst formation is uncommon among bacteria;
most studies on bacterial cyst formation have been carried out
on species of AZOTOBACTER, particularly A. vinelandii.
In Azotobacter spp, encystment can be promoted in vitro by
the provision of substrates such as b-hydroxybutyrate, and it has
been generally supposed that the intracellular accumulation of
PHB is a necessary pre-requisite for cyst formation; however,
it has been proposed that the stimulus for encystment may be
related to the extracellular levels of both carbon and nitrogen
sources [SBB (1986) 18 2328]. During encystment, cells lose
their flagella and become spheroidal; these heavily encapsulated
cells (precysts) typically accumulate PHB. Membranous blebs
develop at the cell surface, and these subsequently detach and
coalesce forming the fragmented outer layer (exine) of the cyst
wall. Later, the cyst wall develops an electron-transparent inner
layer (intine). The cyst wall contains ALGINATE together with
protein and lipid; the exine is particularly rich in polyguluronic
acid (and Ca2+ ), while the intine is richer in polymannuronic
acid. Azotobacter cysts are metabolically dormant, and they can
remain viable in dry soil for many years; they are more resistant
than the vegetative cells to desiccation, sonication and ultraviolet
radiation, but they are not significantly more resistant to heat.
Azotobacter-like lipid cysts are formed by some members
of the Methylococcaceae.
(See also MICROCYST.)
(b) (protozool.) Cysts are formed e.g. by some amoebae,
ciliates and phytoflagellates. During encystment, structures such
as cilia or flagella are lost or resorbed, and considerable
reorganization of internal structures may occur; the cell becomes
enclosed by a thin or thick, commonly multilayered wall, the
outer-most layer(s) being termed the ectocyst or exocyst, the
innermost layer(s) the endocyst, and intermediate layer(s) the
mesocyst. Cyst walls vary in composition, according to species;
they commonly contain a high proportion of protein, while
e.g. cellulose occurs in the endocyst of Acanthamoeba spp,
chitin apparently occurs in Entamoeba cysts [BBRC (1982)
108 815821], and sulphated glycosaminoglycans occur in the
mesocyst in Histriculus similis [JGM (1983) 129 829832].
Cysts of CHRYSOPHYTES have silica walls. (In certain loricate
or testate organisms e.g. Euglypha spp a cyst is formed
when the organism withdraws into its lorica/test and plugs the
aperture.) Excystment (the release of one or more vegetative cells
from the cyst) may involve rupture of the cyst wall (possibly as
a result of the intake of water) and/or enzymic dissolution of the
wall; in e.g. Naegleria gruberi the cell leaves the cyst via a pore
which becomes unplugged, while in Acanthamoeba a lid-like
operculum is removed from an exit aperture in the cyst wall.
In many protozoa the cyst serves a protective function,
allowing the organism to survive e.g. the absence of food,
cytochrome oxidase
some way beyond the tips of the basidia. Their function is largely
unknown; however, those which arise from the surfaces of the
lamellae of certain species of Coprinus appear to function as
spacers maintaining a small but significant distance between
adjacent lamellae, thus facilitating spore dispersal.
cystinelactoseelectrolyte-deficient medium See CLED MEDIUM.
cystinetelluriteblood agar See TELLURITE MEDIA.
cystitis Inflammation of the urinary bladder. Symptoms: frequent,
painful micturition, sometimes with haematuria, fever etc. Cystitis may result from the spread of an infection upwards from the
urethra or downwards from the kidney. The former is more common, with Escherichia coli (see UPEC) and Proteus spp being the
most common causal agents; other causal agents include enterococci and Staphylococcus saprophyticus. Treatment may involve
e.g. copious fluid intake and therapy with broad-spectrum antibiotics.
Certain adenoviruses (e.g. type 11) have been associated with
haemorrhagic cystitis (mainly in children).
(See also URINARY TRACT INFECTION.)
Cystobacter See MYXOBACTERALES.
Cystodinium A genus of DINOFLAGELLATES in which the vegetative cells are unicellular and non-motile, and reproduce by the
formation of zoospores.
Cystomyces See UREDINIOMYCETES.
Cystoseira See PHAEOPHYTA.
cystosorus A cluster of cysts: see e.g. PLASMODIOPHOROMYCETES.
Cystotheca See ERYSIPHALES.
Cystoviridae (f6 phage group) A family of BACTERIOPHAGES
containing one genus (Cystovirus) and one member: BACTERIOPHAGE f6.
Cystovirus See CYSTOVIRIDAE.
cystozoite (bradyzoite) In certain coccidia: a stage within host
tissues (see e.g. TOXOPLASMOSIS).
cytarabine (1-b-D-arabinofuranosylcytosine; ara-C; cytosine arabinoside) An ARABINOSYL NUCLEOSIDE originally investigated as a
possible systemic ANTIVIRAL AGENT for disseminated herpesvirus
infections; toxicity has limited its clinical use.
cytidine See NUCLEOSIDE and Appendix V(b).
cytidine deaminase See RNA EDITING.
cytoadherence See MALARIA.
cytoadhesin subfamily A category within the INTEGRIN family
which includes CD41b/CD61.
cytobiosis SYMBIOSIS in which one symbiont occurs within the
cells of the other.
cytochalasins A family of fungal secondary metabolites (POLYKETIDE derivatives) cytochalasins A, B, C etc. which are
formed e.g. by species of Aspergillus, Helminthosporium and
Phomopsis. Cytochalasins bind to one end of an ACTIN microfilament (the fast-growing or barbed end) and inhibit the addition
of further monomers thus inhibiting e.g. phagocytosis, amoeboid movement, the intracellular development of certain viruses,
and other microfilament-dependent functions. (Cytochalasin B
apparently slows, but does not prevent, the addition of actin
monomers [JCB (1986) 102 282288].) Cytochalasins A and E
enhance branching in certain fungi (see GROWTH (fungal)).
cytochrome See CYTOCHROMES.
cytochrome oxidase In an ELECTRON TRANSPORT CHAIN a (terminal) cytochrome which transfers electrons to molecular oxygen,
reducing it to water. Cytochrome oxidases include cyts aa3 , a1 ,
d and o (see CYTOCHROMES). Bacteria typically have more than
one type of cytochrome oxidase. The electron transport chain
in the animal MITOCHONDRION appears to have only one type
cytokines
a given type of STAT relays the signal for only some type(s)
of cytokine thus permitting different cytokines to initiate
different signals in the same cell. Phosphorylated STATs form
homo- or heterodimers that enter the nucleus and promote
transcription of particular gene(s). [STATs: TIBS (2000) 25
496502.]
As mentioned, a given cytokine may cause diverse effects.
For example, the binding of tumour necrosis factor (TNF) to
its receptor can result in activation of caspases (and APOPTOSIS) or e.g. transcription of specific genes through activation
of a major transcription factor: nuclear factor-kB (NF-kB). In
the latter pathway, the binding of TNF to its receptor promotes
phosphorylation (and consequent degradation) of a certain protein (IkBa) which, by binding to NF-kB, inactivates it; that is,
phosphorylation (degradation) of IkBa results in the activation
of NF-kB. NF-kB is important e.g. in the development of an
inflammatory response; it promotes transcription of a range of
genes including those encoding TNF-a, IL-1b and IL-8.
In general, the binding of cytokines to their receptors may
initiate cellular responses that range from secretion (of cytokines
etc.), differentiation or proliferation to chemotaxis or apoptosis;
currently, many of the signalling pathways in eukaryotic cells are
incompletely understood. [Signalling mechanisms in prokaryotes
and eukaryotes: Book ref. 218, pp 89162; Book ref. 226, pp
111140.]
Note regarding nomenclature of cytokines. The name of
a cytokine does not necessarily correlate with its primary
function(s) in vivo. For example, tumour necrosis factor was
initially identified as an anti-tumour agent but is now known
to be a central mediator in host defence and inflammation.
Again, some interleukins, initially thought to mediate only
leukocyteleukocyte interactions, are now known to involve
other types of cell; thus, e.g. interleukin-8 is secreted by
endothelial cells and is classified as a chemokine.
Cytokines as factors in health and (infectious) diseases. Various roles have been attributed to cytokines in normal physiology and development. However, the contribution of individual
cytokines in vivo has been difficult to establish experimentally not least because of the complexity of the system and the
existence of biochemical redundancy among cytokines; hence,
in some cases, the function(s) of a cytokine have been inferred
from the effects attributed to inherited deficiencies in the synthesis or activity of that cytokine (and/or its receptor). In other
cases, the role(s) of cytokines have been inferred from studies
on knockout mice in which genes of particular cytokine(s) have
been rendered non-functional.
In diseases of microbial aetiology, cytokines typically have
protective roles e.g. in processes such as ANTIBODY FORMATION and INFLAMMATION. However, dysregulation of cytokines
(enhanced production, imbalance, inhibition) may be a major
factor in pathogenesis.
In some cases, the severity of, or susceptibility to, disease
has been found to vary in different individuals according to
the nature of the TNF-a gene promoter particular polymorphisms in the promoter region of the gene being associated with
enhanced production of the cytokine; this has been reported in
cerebral MALARIA [Nature (1994) 371 508510] and in ENDOTOXIC SHOCK [JAMA (1999) 282 561568]. Again, polymorphisms in the gene encoding IL-1b have been associated with an
increased risk of gastric cancer from Helicobacter pylori infection [Nature (2000) 404 398402].
In pyelonephritis caused by Escherichia coli, the cytokines IL6 and IL-8 appear to be prominent levels of IL-6 correlating
cytokinesis
to be down-regulated in naive CD4+ cells [PNAS (1999) 96
30233028].)
Studies carried out in vitro and in vivo suggest that the
cytokines secreted by (Th1 or Th2) cells are responsible for
various aspects of the immune response observed during infections. Thus, inflammatory Th1 cells secrete pro-inflammatory
cytokines that are associated with important roles in cellmediated immunity. For example, IFN-g activates macrophages
which may then (i) exhibit enhanced antimicrobial activity in
phagosomes, (ii) secrete IL-8, attracting immune cells to the site
of infection, and (iii) secrete IL-12, promoting further development of the Th1 subset. Moreover, IFN-g can promote class
switching to complement-fixing, opsonizing antibodies (human
IgG1, IgG3; murine IgG2a). Th1 cytokines can e.g. upregulate
expression of E selectins (see INFLAMMATION) and they can also
upregulate MHC class II antigens. DELAYED HYPERSENSITIVITY is
one manifestation of the characteristically cell-mediated Th1type immune response.
Th2 cells are typically T-helper cells in ANTIBODY FORMATION.
Th2 (anti-inflammatory) cytokines down-regulate macrophages
and promote B cell activation, thus being important in the
humoral (antibody-mediated) immune response to infection by
e.g. extracellular bacteria and helminths etc. IL-4 promotes class
switching to non-complement-fixing IgG (human IgG4; murine
IgG1) as well as to IgE in both man and mice. IL-5 promotes
eosinophilia which may give activity against e.g. helminths and
other parasites. IL-6 may contribute to antimicrobial activity
by stimulating B cell proliferation and/or inducing ACUTE-PHASE
PROTEINS.
Therapeutic uses of cytokines. Because cytokines regulate so
many aspects of the immune defence system they are attractive as candidate therapeutic agents; for example, INTERFERONS
have been useful in various contexts. However, some cytokines
(e.g. TNF), though potentially useful, may be unsuitable for
therapy owing e.g. to instability or toxicity in vivo; interestingly, a non-toxic TNF-mimetic peptide has been found to prevent recrudescence of Mycobacterium bovis (BCG) infection in
CD4+ T cell-depleted mice [JLB (2000) 68 538544]. Inhibition of TNF-a can be achieved by monoclonal antibodies or
by soluble TNF-a receptor molecules. [New perspectives on
the design of cytokines and growth factors: TIBtech. (2000) 18
455461.]
[Molecular biology of the cytokines: Book ref. 226.]
cytokinesis Those events, excluding nuclear division, which
occur during the division of a eukaryotic cell into progeny cells;
they include the apportionment of the cytoplasm and organelles,
and may include e.g. synthesis of new material for the cell wall
of each progeny cell.
cytokinins (kinins, phytokinins) PHYTOHORMONES which stimulate metabolism and cell division; the cytokinins are 6-Nsubstituted adenines which are synthesized mainly at the root
apex and translocated via the xylem. (Cytokinin-like activity is
exhibited by certain urea derivatives, e.g. diphenylurea (found
in coconut milk); it is believed that such compounds act by promoting the 6-N-substitution of endogenous adenine.) The mechanism by which cytokinins promote cell division is unknown;
one suggestion is that cell division is encouraged by an increase
in the level of endogenous cAMP brought about by the inhibition
of cAMP phosphodiesterase by cytokinins.
Compounds similar or identical to cytokinins are produced
by certain microorganisms; such compounds may account for
the formation of ROOT NODULES and for the development of
symptoms in e.g. FASCIATION.
Th1
Interleukin-2
Interleukin-3
Interleukin-4
Interleukin-5
Interleukin-6
Interleukin-10
Interleukin-13
Interferon-g
TNF-a
TNF-b
+
+
+
+
+
Th2
+
+
+
+
+
+
+a
Secretion from Th2 cells reported to be lower than that from Th1
cells.
216
cytoplasmic membrane
the oral cavity in vertebrates (Simonsiellaceae); non-pigmented
filaments, attached (at one end) to other filaments or to the
substratum, which form gliding gonidia (Leucotrichaceae). Genera include ALYSIELLA, BEGGIATOA, CYTOPHAGA, FLEXIBACTER,
HERPETOSIPHON, LEUCOTHRIX, SAPROSPIRA, SIMONSIELLA, SPOROCYTOPHAGA, THIOPLOCA, THIOTHRIX and VITREOSCILLA.
In another taxonomic scheme [ARM (1981) 35 339364 cf.
FLEXIBACTERIAE], of the above genera only Cytophaga, Flexibacter and Sporocytophaga are included in the Cytophagales; the
other genera are classified as apochlorotic cyanobacteria.
cytopharyngeal apparatus (ciliate protozool.) Skeletal and certain other elements of the CYTOPHARYNX. Two main types of
cytopharyngeal apparatus have been distinguished: the CYRTOS
and the RHABDOS; this taxonomically important distinction is
believed to reflect evolutionary differences in the different ciliate
groups those having a rhabdos-type structure being regarded
as the more primitive.
cytopharyngeal basket Syn. CYRTOS.
cytopharynx (ciliate protozool.) An invagination of the cytoplasmic membrane which is supported, within the cytoplasm,
by a tubelike system of microtubules and/or microfibrils. (See
also CYTOPHARYNGEAL APPARATUS and CYTOSTOME.) Food particles which pass into the (non-ciliated) cytopharynx are taken
up by PHAGOCYTOSIS through the cytoplasmic membrane at its
inner end.
cytophilic antibodies Antibodies which can bind to a cell surface
without involving their COMBINING SITES; the bound antibody
can therefore still bind homologous antigen. (See e.g. REAGINIC
ANTIBODIES.)
cytoplasmic genes (extrachromosomal genes; extranuclear genes)
Genes which are not located on a bacterial CHROMOSOME
or in a (eukaryotic) NUCLEUS; in eukaryotic organisms the
term commonly refers to the genes in a CHLOROPLAST or a
MITOCHONDRION, while in prokaryotes it has been used to refer
to the genes carried by a PLASMID. (See also CYTOPLASMIC
INHERITANCE.)
cytoplasmic heterozygote See CYTOHET.
cytoplasmic inheritance (extrachromosomal inheritance; nonMendelian inheritance) Inheritance governed or influenced by
CYTOPLASMIC GENES which are not subject to the Mendelian
laws of segregation and assortment; see e.g. MATERNAL
INHERITANCE.
cytoplasmic membrane (CM; cell membrane; plasma membrane;
plasmalemma; protoplast membrane) The lipid- and proteincontaining, selectively permeable membrane which encloses the
cytoplasm in prokaryotic and eukaryotic cells; in most types of
microbial cell the CM is bordered externally by the CELL WALL. In
microbial cells the precise composition of the CM may depend
on growth conditions and on the age of the cell.
The structure of all biological membranes appears to conform to the basic fluid mosaic model. In this model the lipid
molecules form a bilayer within which the protein molecules
are partly or wholly embedded some spanning the entire width
of the bilayer; the lipid molecules are orientated such that their
polar groups form the outer, hydrophilic surfaces of the bilayer
while their hydrocarbon chains form the hydrophobic interior of
the bilayer. (cf. UNIT MEMBRANE.) The membrane proteins are
sometimes categorized as either peripheral (= extrinsic) proteins (bound to the membrane e.g. by electrostatic forces, and
easily removable by electrolytes or chelating agents) or integral (= intrinsic) proteins (bound more strongly by hydrophobic
bonds and extractable, with difficulty, by detergents or organic
solvents). Cytoplasmic membranes are characteristically asymmetrical, i.e. the components of the outer (externally facing)
Interestingly, cytokinins are incorporated in specificitydetermining positions in a small proportion of tRNA molecules.
(See also KINETIN and ZEATIN.)
cytolysin A toxin which lyses (usually eukaryotic) cells.
cytolytic Able to lyse cells.
cytolytic T cell See T LYMPHOCYTE.
cytomegalic inclusion disease (CID) A disease caused by human
cytomegalovirus (CMV) see BETAHERPESVIRINAE. CMV can
infect almost any tissue; infected cells are characteristically
enlarged with large intranuclear inclusion bodies. Virus transmission occurs e.g. by direct contact, by transfusion of blood
from an infected donor, or via the placenta. Congenital CID is
commonly asymptomatic, but can be a severe condition with e.g.
hepatosplenomegaly, encephalitis with irreversible CNS damage, and increased incidence of congenital deformities (see also
TORCH DISEASES). Postnatal and adult infections are probably
largely asymptomatic; in some cases the disease resembles INFECTIOUS MONONUCLEOSIS (CMV mononucleosis, PaulBunnell
test negative). In immunodeficient patients CMV infection may
lead to e.g. pneumonia, transplant rejection, and/or death; infection may be primary or may result from reactivation of latent
CMV. Patients at risk from CMV-related disease may be monitored by a NASBA-based assay of cytomegalovirus late gene UL65
(which encodes the pp67 protein) [JCM (1998) 36 13411346];
a commercial form of the assay for CMV was introduced
by Organon Teknika. Known antiviral agents are not effective
against CID.
cytomegaloviruses See BETAHERPESVIRINAE.
cytomegaly See CYTOPATHIC EFFECT.
cytomembranes Syn. INTRACYTOPLASMIC MEMBRANES.
cytomere A multinucleate structure which is formed by fragmentation of a schizont and which subsequently gives rise to
merozoites.
cytopathic effect (CPE) (virol.) A change or abnormality in cells
due to virus infection. CPEs may include e.g. INCLUSION BODY
formation, cytoplasmic vacuolation (see e.g. SPUMAVIRINAE),
cell enlargement (cytomegaly) (see e.g. BETAHERPESVIRINAE),
SYNCYTIUM formation (see e.g. PARAMYXOVIRUS), the formation
of discrete foci of cell proliferation (see e.g. FRIEND VIRUS and
MCF VIRUSES), cell death (see also PLAQUE), etc. The CPEs
produced by a given virus in a given cell system are often
characteristic and may be useful in the identification of the virus;
some viruses characteristically fail to give rise to CPE even when
viral replication occurs (see e.g. RUBIVIRUS).
Cytophaga A genus of GLIDING BACTERIA of the CYTOPHAGALES;
species occur in soil and in freshwater, estuarine and marine
habitats. The organisms are rods or filaments, up to ca. 50 m
long, containing carotenoid pigments ranging from yellow to
red; they are chemoorganotrophs and may be aerobic (respiratory metabolism using oxygen or, in at least one strain,
nitrate as electron acceptor) or facultatively anaerobic (facultatively fermentative). Typically, Cytophaga spp can attack
polysaccharides such as AGAR, ALGINATE, CELLULOSE and CHITIN.
GC%: ca. 2839.
Cytophagaceae See CYTOPHAGALES.
Cytophagales An order of GLIDING BACTERIA which do not form
fruiting bodies (cf. MYXOBACTERALES); constituent species, all
of which are Gram-negative, occur e.g. in soil and in freshwater, estuarine and marine habitats. In an early taxonomic
scheme [Book ref. 21, pp. 99119] four families were distinguished: motile rods or filaments containing carotenoid pigments
(Cytophagaceae); motile filaments lacking carotenoid pigments
(Beggiatoaceae); flat, non-pigmented, motile filaments found in
217
cytoplasmic membrane
Lipid components of bacterial CMs are mainly phospholipids;
in many or all cases, these are synthesized within the membrane
itself.
Phosphatidylglycerols (PG) appear to occur in all bacteria, while phosphatidylethanolamine (PE) is more common and
more abundant in Gram-negative species; phosphatidylcholine is
absent in Gram-positive cells and is rare in Gram-negative bacteria. Phosphatidylinositol occurs in some bacteria (e.g. Mycobacterium spp). PLASMALOGENS are found in the cytoplasmic membrane in some anaerobes. In Escherichia coli the main phospholipid is PE PG and diphosphatidylglycerol (DPG, cardiolipin)
being relatively minor components.
Glycolipids are common in small quantities; in some Grampositive bacteria molecules of glycolipid may be covalently
linked to glycerol TEICHOIC ACIDS, forming lipoteichoic acid.
Sphingolipids are rare in bacterial membranes.
Sterols are absent in most species (cf. MYCOPLASMATACEAE).
Hopanes (triterpene derivatives which resemble sterols in size,
rigidity and amphiphilicity) are present in some bacteria [JGM
(1985) 131 13631367].
Lipoamino acids (O-aminoacylphosphatidylglycerols) occur
in the membranes of some Gram-positive bacteria (e.g. Bacillus
spp, Clostridium spp, Staphylococcus aureus). These are esters
of PG and basic amino acids such as arginine, lysine or ornithine;
the proportion of lipoamino acids varies according to growth
phase and to the pH of the medium.
The CM fatty acids may be straight-chained or branched
(the latter more common in Gram-positive species), saturated
or unsaturated; some contain a cyclopropane ring (which is
formed by methylation at a double bond). Phospholipids often
contain one saturated and one unsaturated fatty acid residue per
molecule.
In E. coli the main saturated fatty acids are hexadecanoic
(palmitic) and tetradecanoic (myristic) acids, minor components
including e.g. octadecanoic (stearic) and dodecanoic (lauric)
acids; the main unsaturated fatty acids (all of which are cismonoenes) include e.g. cis-19 -hexadecenoic (palmitoleic) acid.
In general, the CM varies in its fatty acid composition
according to growth conditions (e.g. temperature, pH). Thus, in
some species the proportion of unsaturated fatty acids increases
when the growth temperature decreases e.g. in E. coli the
proportion of unsaturated fatty acids increases from 16% to 49%
when the growth temperature falls from 36 C to 25 C; such
a change appears to be a compensatory response which helps
to maintain optimum membrane fluidity. In contrast, almost
no increase in monoenoic fatty acids occurs in the CM of
Staphylococcus aureus when the growth temperature drops from
37 C to 25 C [Book ref. 44, p 402]. In some bacteria, adaptation
to lower growth temperatures involves an increase in the length
of fatty acid chains rather than an increase in the degree of
unsaturation [JGM (1985) 131 22932302].
The lipids of the CM clearly contribute to the essential feature
of selective permeability. However, the lipids also have other
functions; for example, in E. coli phosphatidylethanolamine can
behave as a molecular chaperone, being required for the correct
folding (maturation) of the membrane protein LacY [EMBO
(1998) 17 52555264].
Proteins in the bacterial CM include a variety of enzymes
(involved e.g. in the synthesis of phospholipids and cell wall
components); for example, penicillin-binding proteins (involved
in the synthesis of PEPTIDOGLYCAN) may form part of a protein
complex in the CM [FEMS Reviews (1994) 13 112]. There
are also components of TRANSPORT SYSTEMS, energy-converting
cytoskeleton
systems (see e.g.
PLASMIC OXIDATION)
219
cytosol
[Molecular biology of the cytoskeleton: Book ref. 166; in vitro
translocation of organelles along microtubules: Cell (1985) 40
729730; reviews: JCS (1986) Supplement 5; the cytoskeleton
in protists: Int. Rev. Cytol. (1986) 104 153249.]
cytosol The fluid (non-particulate) fraction of cytoplasm. (cf.
CELL SAP; HYALOPLASM.)
cytostome In certain protozoa (including many ciliates and some
others, e.g. Noctiluca, Peranema): the cell mouth, a specific
region of the cell through which particulate food is ingested.
(See also AMOEBOSTOME.)
In ciliates the cytostome is regarded as a two-dimensional
aperture at the level of the PELLICLE; in this region the pellicle
lacks both cilia and pellicular alveoli, and is typically invaginated within a supportive collar or tube-like structure of microtubules and/or microfibrils in the cytoplasm (see also CYTOPHARYNX and CYTOPHARYNGEAL APPARATUS). In advanced ciliates
(e.g. Paramecium) that part of the pellicle which includes the
220
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
D
D
TRNA).
AMINO
ACIDS).
ostiolar pores at the surface. The bulk of the stromal tissue may
act as a reservoir for water. (See also ASCOSPORE.)
Dalmau plate technique A technique used e.g. for studying the
formation of pseudomycelium or true mycelium by a yeast. A
streak and two point-inoculations of the test strain are made
at well-separated locations on a surface-dried plate of e.g.
CORNMEAL AGAR; the centre of the streak and one of the pointinoculations are then each overlaid with a sterile cover-glass.
After incubation at 25 C for ca. one week the preparation is
examined under the microscope.
Dalmeny disease A disease of cattle which results in e.g.
abortion or death; the causal agent is believed to be a species of
SARCOCYSTIS.
dalton (Da) Syn. ATOMIC MASS UNIT.
Dalyellia viridis See ZOOCHLORELLAE.
Dam-directed mismatch repair See MISMATCH REPAIR.
dam gene
In e.g. Escherichia coli : a gene which encodes
a DNA adenine methylase (Dam methylase), i.e. an enzyme
that methylates DNA at the N-6 position of adenine in the
nucleotide sequence 5 -GATC-3 (Dam site); a strand of DNA
is methylated soon after its synthesis (see DNA METHYLATION).
Dam methylation is involved e.g. in MISMATCH REPAIR in
E. coli. It is also involved in regulating certain genes. For
example, transposition of the transposon Tn10 (q.v.) is inhibited
by Dam methylation of a sequence in the transposase gene
promoter (reducing transposase synthesis) and of a sequence
in IS10 (reducing transposase activity); Tn10 transposition is
thus apparently coupled to DNA replication: it occurs just after
the replication fork has passed but before Dam methylation has
occurred.
Other genes which contain Dam sites in their promoters, and
whose expression is sensitive to Dam methylation, include e.g.
the trpR gene of E. coli, the cre gene of BACTERIOPHAGE P1, and
the mom gene of BACTERIOPHAGE MU. The chromosomal origin,
oriC, in E. coli contains more than 10 Dam sites which may
be important in regulating the initiation of DNA replication (see
CELL CYCLE (b)).
[Minireview: JB (1985) 164 490493.]
Dam methylation apparently occurs in various other Gramnegative bacteria (including certain cyanobacteria) and in some
members of the Archaea.
Dam methylation See DAM GENE.
damping off (plant pathol.) A microbial disease of seedlings in
which e.g. roots may rot, or the hypocotyl (lower stem) may
either collapse or become wiry (wire stem); seedlings may
die before or after they emerge from the soil (pre-emergence
and post-emergence damping off, respectively). Common causal
agents include species of PYTHIUM and RHIZOCTONIA. Aerial parts
are often secondarily affected by GREY MOULD. Damping off
may be controlled e.g. by CARBENDAZIM, CHESHUNT COMPOUND,
CHLORONEB or ETRIDIAZOLE. (cf. FOOT-ROT (sense 2) and BLACKLEG (sense 2).)
Dane particle See HEPATITIS B.
DanielliDavson model See UNIT MEMBRANE.
Danish agar Syn. FURCELLARAN.
danofloxacin See QUINOLONE ANTIBIOTICS.
dansyl chloride A reagent, 5-(dimethylamino)naphthalene-lsulphonyl chloride, which reacts with amino acids and proteins
to form derivatives that exhibit an intense yellow fluorescence
under UV irradiation.
Danysz phenomenon The phenomenon in which the residual
toxicity in a mixture of diphtheria toxin and antitoxin varies
according to the method of admixture. Thus, if toxin is added to
222
defective virus
an S LAYER. Carbohydrate chains originating at the outer membrane pass through the S layer and form the outermost surface
of the cell. The S layer also called the HPI (= hexagonally
packed intermediate) layer is composed of a single polypeptide species. [Three-dimensional structure of the HPI layer: JMB
(1986) 187 241253.] D. radiodurans does not contain phosphatidylglycerol or phospholipids derived from it. [Polar lipid
profiles of Deinococcus: IJSB (1986) 36 202206.] The genome
is toroidal [Science (2003) 299 254256].
Dekkera
A genus of yeasts (family SACCHAROMYCETACEAE)
which reproduce by budding; pseudomycelium is usually
formed. Asci are evanescent and are formed directly from
(diploid) vegetative cells; ascospores are more or less bowlerhat-shaped, 14 per ascus. NO3 may or may not be assimilated.
Two species: D. bruxellensis (anamorph: Brettanomyces bruxellensis) and D. intermedia (anamorph: B. intermedius), found in
beers, wines etc. (See also BRETTANOMYCES.) [Book ref. 100,
pp. 146150.]
delavirdine See ANTIRETROVIRAL AGENTS.
delayed enrichment method See AUXOTROPH.
delayed hypersensitivity (DH; delayed-type hypersensitivity; cellmediated hypersensitivity; type IV reaction) (immunol.) In a
PRIMED individual: a HYPERSENSITIVITY (sense 1) response which
(i) follows the second (or subsequent) exposure to the given
antigen, (ii) is mediated by antigen-specific T LYMPHOCYTES,
and (iii) involves a local inflammatory reaction that reaches
maximum intensity 2448 hours after antigenic challenge. (cf.
IMMEDIATE HYPERSENSITIVITY.)
Priming and subsequent antigenic challenge may occur in
the skin or elsewhere. Initial priming (or sensitization), in
which the individual is initially exposed to the given antigen,
involves interaction between an ANTIGEN-PRESENTING CELL (e.g. a
DENDRITIC CELL) and an antigen-specific CD4+ T cell. The T cell
forms a Th1 clone: when activated by antigen it proliferates and
secretes CYTOKINES that include INTERLEUKIN-2. Hence, a primed
individual contains an expanded clone of specifically reactive
T cells (referred to as TDH , TDTH or Tdth). Sensitization may
require a period of 12 weeks.
Following sensitization, a DH reaction can be elicited by
further exposure to specific antigen; as before, antigen is
presented by an APC, but in this instance the (primed) individual
contains an expanded clone of specifically reactive T cells. The
secreted cytokines include e.g. interleukin-2, INTERLEUKIN-12 and
IFN-g (see INTERFERONS); the cytokines (i) promote expansion of
the Th1 subset of T cells (which secrete more pro-inflammatory
cytokines) and (ii) bring about the accumulation of activated
MACROPHAGES at the site of antigenic challenge. In the skin, the
result is typically an indurated (hard), erythematous (red) nodule
which develops in 2448 hours of antigenic challenge.
The lesion commonly resolves slowly. However, when there
is a failure to eliminate the antigen (or pathogen) the ongoing
presence of a concentration of activated macrophages can result
in damage to the hosts tissues. In some diseases aggregations
of macrophages give rise to epithelioid cells and, subsequently,
GIANT CELLS within lesions called GRANULOMAS; tubercles are
granulomas formed in tuberculosis.
DH to a given antigen can be transferred to a non-primed
subject only by the transfer of cells, not serum or plasma alone.
(cf. JONESMOTE SENSITIVITY.)
DH reactions can be modified by various drugs; for example,
glucocorticosteroids can inhibit DH reactions, and certain antitumour agents, such as mitomycin C, have been found to stimulate
DH reactions in mice.
dendritic cells
to develop stable and heritable resistance to B. thuringiensis
crystals within a few generations [Science (1985) 229 193195].
(cf. THURINGIENSIN.)
[Reviews: Book ref. 171, pp. 185209 (commercial aspects),
pp. 211249 (genetics of B. thuringiensis); MR (1986) 50
124.]
(cf. MILKY DISEASE.)
d-factor See RNA POLYMERASE.
delta hepatitis virus See DELTA VIRUS.
delta herpesvirus A herpesvirus which is antigenically related
to human varicella-zoster virus (see ALPHAHERPESVIRINAE) and
which causes a varicella-like disease in non-human primates.
delta particles See TECTIBACTER.
delta plasmid See DELTA.
d sequence See TY ELEMENT.
delta transfer factor See DELTA.
delta virus (delta agent; hepatitis D virus; hepatitis delta virus)
A defective RNA virus which can replicate only in the presence
of a helper virus of the HEPADNAVIRIDAE usually HEPATITIS B
VIRUS (HBV), although under experimental conditions the delta
virus can replicate in woodchucks infected with WOODCHUCK
HEPATITIS VIRUS. The delta virus virion (as derived from the serum
of an HBV-infected patient) is ca. 3537 nm in diam.; it consists
of a core containing the delta virus RNA genome (MWt ca.
5.5 105 ) and a delta virus-encoded protein antigen (HDAg)
surrounded by an (HBV-encoded) HBsAg-containing envelope.
The genome is circular ssRNA [PNAS (1986) 83 87748778].
[Protein composition of the delta virus virion: JV (1986) 58
945950.]
In humans, the delta virus can infect an individual either
simultaneously with HBV or subsequent to the establishment
of an HBV infection; delta virus infection may itself be acute
or chronic. The presence of the delta virus may exacerbate the
symptoms of HBV infection, in some cases inducing an acute,
severe or fulminant hepatitis particularly when an acute delta
virus infection is superimposed on a pre-existing chronic HBV
infection. HDAg can be detected in the serum of the patient only
very early in infection, but anti-HDAg antibodies apparently
persist indefinitely in chronically infected patients; evidence
of active delta virus replication requires immunohistological
staining for HDAg in the hepatocytes.
1GATP See CHEMIOSMOSIS.
1Gp See CHEMIOSMOSIS.
H+ See CHEMIOSMOSIS.
1m
1p See CHEMIOSMOSIS.
1pH See CHEMIOSMOSIS.
1y See CHEMIOSMOSIS
dematiaceous (mycol.) Darkly pigmented.
demeclocycline See TETRACYCLINES.
demecolcine Deacetyl-N-methyl-COLCHICINE.
Demerec convention A widely-followed convention for bacterial
genetic nomenclature [Genetics (1966) 54 6176].
demethylchlortetracycline See TETRACYCLINES.
demicyclic rusts Those rust fungi (see UREDINIOMYCETES) which
form all types of spore except uredospores; they include e.g.
most species of Gymnosporangium.
demyelination (demyelinization) The removal or destruction of
the myelin sheath of one or more nerve fibres. (See also MULTIPLE SCLEROSIS; PROGRESSIVE MULTIFOCAL LEUKOENCEPHALOPATHY;
VISNA.)
denaturing gradient gel electrophoresis See DGGE.
Dendriscocaulon See CEPHALODIUM.
dendritic cells Motile, non-phagocytic ADHERENT CELLS, derived
from the bone marrow, which are present e.g. in spleen and
dendrodochiotoxicosis
(See also NITROGEN CYCLE).
denitrifying bacteria Those bacteria capable of DENITRIFICATION;
they occur e.g. in soil and in marine and freshwater environments. (Some species can be useful in the elimination of nitrate
from waste water.) Examples include e.g. Bacillus licheniformis,
Hyphomicrobium sp, Paracoccus denitrificans, Pseudomonas
stutzeri and Thiobacillus denitrificans.
density gradient centrifugation See CENTRIFUGATION.
densonucleosis viruses See DENSOVIRUS.
Densovirus (insect parvovirus group; also: densonucleosis viruses,
DNVs) A genus of autonomous (helper-independent) viruses
(family PARVOVIRIDAE) which infect insects of the Lepidoptera
(and probably of the Diptera and Orthoptera). Both positive- and
negative-strand ssDNA molecules are encapsidated (in separate
virions). Replication occurs in most tissues of host larvae,
nymphs and adults; hypertrophy of the nucleus occurs in infected
cells, and virions accumulate in dense intranuclear inclusions.
Infected insects may die. Type species: densovirus of Galleria
mellonella (the greater wax moth, whose larvae known as waxworms feed on pollen and wax in beehives). Other members
include densovirus of Junonia (a genus of butterflies); similar
viruses have been detected in e.g. Aedes (mosquitoes), Bombyx
(silk-moth), and butterflies of the Nymphalidae.
dental caries Tooth decay: typically, a process in which acids
(particularly lactic acid), formed by plaque microorganisms,
cause localized breakdown (demineralization) of tooth enamel,
thus exposing the dentine; an important factor in the development of caries is the formation of water-insoluble extracellular
microbial glucans which promote adhesion of cariogenic bacteria to the tooth surfaces (see DENTAL PLAQUE). Various bacteria,
including e.g. lactobacilli and Streptococcus mutans, can be cariogenic in man; the development of carries may depend on factors
such as the nature of the plaque microflora, diet, and the level
of immunity in the host (see also CREVICULAR FLUID).
Fluoride is a potent anti-caries agent. It converts the apatite
in tooth enamel to the more stable (acid-resistant) fluorapatite,
and this is believed to be the primary mode of fluoride anticaries activity. Fluoride can also inhibit bacterial metabolism
e.g. by blocking the uptake of sugars by the PEP-dependent
phosphotransferase system (see FLUORIDES). However, in some
oral streptococci (including S. mutans) there is an alternative,
fluoride-insensitive, pmf-dependent uptake system for glucose;
this is a low-affinity uptake system compared to the high-affinity
PTS system (the latter operating as a scavenger system under
conditions of substrate limitation). At low pH (e.g. 5.5) the
fluoride-insensitive system appears to be more important than
the PTS system for the uptake of glucose.
dental plaque On the surfaces of teeth: a thin film (up to ca.
0.5 mm thick) consisting of a mixed microbial flora embedded
in a matrix composed largely of extracellular (capsular) bacterial
polysaccharides and salivary polymers; it is a predisposing factor
in DENTAL CARIES and PERIODONTITIS.
Early colonizers of a clean enamel surface (in man) include
species of Neisseria and Streptococcus (particularly S. sanguis).
If plaque is allowed to build up, the nature of the microflora
changes with time; although streptococci tend to remain dominant, anaerobes and filamentous bacteria begin to appear in significant numbers after several days or a week. Organisms present
in well-established plaque include e.g. species of ACTINOMYCES
(particularly A. viscosus), BACTEROIDES and VEILLONELLA; there
is a general correlation between the numbers of Streptococcus
mutans (see STREPTOCOCCUS) and the dietary intake of sucrose.
The nature of the plaque microflora varies e.g. from one individual to another, and from one site to another on a given tooth.
lymph nodes. Dendritic cells are irregularly shaped, smoothsurfaced cells which contain pulsatile nuclei and many spherical
mitochondria; they bear class II MHC antigens (cf. LANGERHANS
CELLS) and can act as ANTIGEN-PRESENTING CELLS (see e.g.
DELAYED HYPERSENSITIVITY) and as accessory cells for cytotoxic
T cells. [Minireviews: Cell (2001) 106 255274.]
dendrodochiotoxicosis (myrotheciotoxicosis) A MYCOTOXICOSIS,
affecting domestic animals and man, caused by roridin and
verrucarin TRICHOTHECENES produced by Myrothecium spp.
Dendrophoma See SPHAEROPSIDALES.
Dendrosoma See SUCTORIA.
dengue (breakbone fever) An acute, tropical and subtropical
human disease caused by any of four serotypes of dengue virus
(family FLAVIVIRIDAE) and transmitted by mosquitoes (usually
Aedes aegypti ). (The genetic diversity of dengue virus is
reported to be increasing, and strains of the virus may now,
or in the future, exhibit differences in virulence [TIM (2000)
8 7477].) Replication of the virus may occur chiefly in
macrophages.
In most cases the disease is benign and self-limiting (dengue
fever ). After an incubation period of 510 days, typical
symptoms include fever, headache, joint and muscular pains, and
(often) a rash; bleeding (e.g. haematuria or gingival bleeding) is
present in some cases. Mortality rates for this classical form
of the disease are very low.
Less often, a more severe form of disease may develop:
dengue haemorrhagic fever (DHF). The manifestations of DHF
include high fever, haemorrhagic phenomena, hepatomegaly
and thrombocytopenia. The severity of disease is influenced
by the extent of plasma leakage (as indicated by the rise in
haematocrit reading). The most severe forms of DHF (World
Health Organization grades III and IV) are designated dengue
shock syndrome (DSS). DSS develops suddenly, after several
days fever, with signs of circulatory failure/hypovolaemic shock
(rapid, weak pulse, narrowed pulse pressure or hypotension, and
cold clammy skin); death may occur in 1224 hours without
suitable treatment, but recovery may be rapid following volumereplacement therapy.
[Dengue haemorrhagic fever (review): RMM (1995) 6 3948.]
In common with many other diseases caused by arthropodborne viruses, various manifestations of dengue infection
(including those in which there is little or no haemorrhage) are
characterized by a transient leukopenia [dengue-induced suppression of bone marrow: BCH (1995) 8 249270]. [Haematology of dengue fever and dengue haemorrhagic fever: BCH
(2000) 13 261276.]
Detection of dengue virus in samples of serum can be achieved
by rtPCR; in primary infection, detection of viral RNA seems
to be optimal prior to seroconversion (soon after onset of
symptoms) [JCM (1999) 37 25432547].
denitrification Energy-yielding (respiratory) metabolism in
which nitrate or nitrite (as terminal electron acceptor) is
sequentially reduced to gaseous products, mainly dinitrogen
and/or nitrous oxide (cf. DISSIMILATORY NITRATE REDUCTION). It is
generally stated that denitrification occurs only under anaerobic
or microaerobic conditions; however, aerobic denitrification
has been reported [AvL (1984) 50 525544; denitrification in
Rhizobium: SBB (1985) 17 19].
In some DENITRIFYING BACTERIA (e.g. Paracoccus denitrificans) electrons from e.g. NADH are transferred to NO3 via a btype cytochrome, and to NO2 and N2 O via c-type cytochromes;
electron flow to NO3 , NO2 and N2 O apparently generates
proton motive force. Nitrate reductase is a MOLYBDOENZYME; in
some species cytochrome d1 c acts as a nitrite reductase.
226
Dermatocarpon
Bacterial polymers typically present in plaque include MUTAN
and LEVANS.
The presence of plaque can be detected by rinsing the mouth
with a solution of a dye (disclosing agent) such as erythrosin.
Dentalina See FORAMINIFERIDA.
deodorants (skin) See SKIN MICROFLORA.
5 -deoxyadenosylcobalamin See VITAMIN B12 .
deoxycholate A salt of deoxycholic acid (see BILE ACIDS).
deoxycholatecitrate agar See DCA.
deoxycholic acid See BILE ACIDS.
deoxycoformycin Syn. pentostatin (see VIDARABINE).
2 -deoxy-2 -fluoro-5-methyl-1-b-D-arabinosyluracil See FMAU.
deoxyhemigossypol A terpenoid PHYTOALEXIN produced by the
cotton plant. [Role of terpenoid phytoalexins in the resistance
of a cultivar of Gossypium barbadense to Verticillium dahliaeinduced wilt: PPP (1985) 26 209218.]
deoxynivalenol See TRICHOTHECENES.
deoxyribonuclease (DNase; DNAase) An enzyme which depolymerizes DNA. A DNase is designated DNase I (EC 3.1.21.1)
or DNase II (EC 3.1.22.1) according to whether the mono- or
oligonucleotide products of its action have (terminal) 5 - or 3 phosphate groups, respectively. DNases are produced e.g. by the
pancreas and by many microorganisms.
In staphylococci, production of a thermostable, Ca2+ requiring, extracellular DNase (thermonuclease: a 5 phosphodiesterase with both endo- and exonuclease activity,
yielding 3 -nucleotides) correlates closely with the production
of COAGULASE; thermonuclease also has Ca2+ -dependent RNase
activity. (Many coagulase-negative staphylococci produce a
DNase which is generally heat-labile.) DNase activity may
be detected/assayed e.g. by measuring changes in turbidity,
or increasing levels of acid-soluble nucleotides (measured by
spectrophotometry at 260 nm), induced in a suspension of DNA.
For the detection of DNase production on solid media, an
agar medium (e.g. trypticasesoy agar) containing DNA and
a calcium salt is inoculated with the test strain and incubated
for 1824 hours. The plate is then flooded with 1 N HCl to
precipitate DNA. A clear zone (in which the DNA has been
hydrolysed) surrounds each DNase-producing colony. Certain
dyes e.g. methyl green (which combines only with highly
polymerized DNA) may be used instead of HCl, in which case
cell viability may be preserved. [Book ref. 44, pp. 757768.]
Certain Clostridium spp produce DNases: e.g. the b-toxins of
C. chauvoei and C. septicum.
See also STREPTODORNASE.
deoxyribonucleic acid See DNA.
deoxyribonucleoside See NUCLEOSIDE.
deoxyribophage A BACTERIOPHAGE with a DNA genome.
deoxyribovirus A VIRUS with a DNA genome.
2-deoxystreptamine 2-Deoxy-1,3-diaminoinositol, a component
of many AMINOGLYCOSIDE ANTIBIOTICS.
DEPC DIETHYLPYROCARBONATE.
Dependovirus (adeno-associated viruses, AAVs; adeno-satellite
viruses) A genus of defective viruses (family PARVOVIRIDAE)
which are totally dependent on functions of a co-infecting helper
adenovirus (or herpesvirus) for their replication. Dependoviruses
can infect a wide range of vertebrate hosts. Type species: AAV-1
(AAV type 1), which infects mainly monkeys; other members:
AAV-2 and AAV-3 (which can infect man), AAV-4 (common
e.g. in African green monkeys), avian AAV, bovine AAV
and canine AAV. (Equine AAV and ovine AAV are probable
members of the genus.) In vitro, a given AAV seems able to
replicate in any type of cell culture which can support the
replication of a suitable helper virus.
dermatomycosis
capitis, FAVUS). Zoophilic dermatophytes commonly show some
degree of host specificity: e.g., M. canis (e.g. cats and dogs),
T. verrucosum (e.g. cattle, horses, pigs, goats), T. equi (horses);
most or all zoophilic species can also infect man. Certain species
(e.g. M. gypseum, T. ajelloi ) are said to be geophilic: they
apparently grow as saprotrophs (e.g. in soil, birds nests), but
can also infect man and animals under certain conditions.
dermatophytosis Syn. RINGWORM.
Dermocarpa A genus of unicellular CYANOBACTERIA (section II)
in which the vegetative cells are rounded and variable in size;
baeocytes initially lack a fibrous outer cell wall layer and are
motile (by gliding). GC%: ca. 3844.
Dermocarpales Syn. Chamaesiphonales (see CYANOBACTERIA).
Dermocarpella
A genus of unicellular CYANOBACTERIA (section II) in which growth and binary fission result in pear-shaped
aggregates consisting of one or two basal cells and a larger apical
cell; multiple fission of the apical cell yields baeocytes which
initially lack a fibrous outer cell wall layer and are motile (by
gliding). GC%: ca. 45.
Dermocystidium See PERKINSUS.
dermonecrotic Causing necrosis of the skin.
dermonecrotic toxin A TOXIN produced by species of Bordetella;
its role (if any) in the pathogenesis of WHOOPING COUGH has not
been determined, but it is known to cause e.g. re-arrangement
of actin filaments within eukaryotic cells.
dermotropism See TROPISM (sense 2).
Derricks method See IMMUNOSORBENT ELECTRON MICROSCOPY.
Derxia
A genus (incertae sedis) of Gram-negative, aerobic,
catalase-negative, chemoorganotrophic, facultatively chemolithoautotrophic bacteria which occur e.g. in acidic tropical soils
(e.g. in Brazil, China, Indonesia, West Bengal). Cells: typically
round-ended pleomorphic rods, ca. 1.01.2 3.06.0 m, with
a single flagellum at one pole (or sometimes at each pole).
Metabolism is respiratory (oxidative), with O2 as terminal
electron acceptor. Carbon sources include glucose, fructose,
ethanol and mannitol; little or no growth occurs on acetate,
lactate, malate or succinate. NITROGEN FIXATION can occur
under atmospheric conditions. Chemolithoautotrophic growth
can occur with mixtures of H2 , CO2 and O2 (CO2 being fixed
via the Calvin cycle), N2 or NH4 + serving as a source of
nitrogen; growth on CH4 or CH3 OH (see METHYLOTROPHY)
has been reported. A pellicle is formed in liquid media;
broth cultures become gelatinous. Colonies are slimy, becoming
raised, wrinkled, and subsequently dark brown. Optimum growth
temperature: 2535 C. Growth occurs within the pH range 5.5ca. 9.0. GC%: ca. 6973. Type species: D. gummosa.
[Book ref. 22, pp. 321325.]
desensitization (syn. hyposensitization) (immunol.) The repeated
administration of known quantities of allergen to an individual
in whom it usually provokes an immediate or delayed
HYPERSENSITIVITY reaction; in some cases this treatment
temporarily reduces or abolishes hypersensitivity to the given
allergen. In one method used for treating allergy to mould(s),
an aqueous extract of the allergen(s) up to 100-fold weaker
than that required to produce an intradermal hypersensitivity
reaction is administered subcutaneously; the dose, initially
given weekly, is gradually increased and administered after
longer intervals of time for a total period of several years [Book
ref. 51, pp. 187201].
Little is known about the mechanism(s) of desensitization.
Possible mechanisms include e.g. (i) the formation of BLOCKING
ANTIBODIES (sense 2), and (ii) the stimulation of suppressor T
cells.
Desulfobulbus
desert fever Syn. COCCIDIOIDOMYCOSIS.
Desert Shield virus See SMALL ROUND STRUCTURED VIRUSES.
desferrioxamine A hydroxamate SIDEROPHORE formed e.g. by
Streptomyces pilosus. It is used e.g. in the treatment of patients
with iron overload.
desiccation (of microorganisms) The removal of water: a process
used e.g. for the PRESERVATION of viable populations of certain
types of microorganism (including enterobacteria and sporeforming bacteria). However, the method described below is
lethal for many types of microorganism, including various
pathogens (e.g. Neisseria gonorrhoeae, Treponema pallidum)
and many aquatic organisms; some organisms that are killed
by this procedure can be preserved by FREEZE-DRYING.
Initially, the organisms are suspended in an appropriate
medium (e.g. broth, serum, or 510% nutrient gelatin). Drops
of the suspension are then placed, singly, onto a sterile filter
paper (or a piece of waxed paper) which is inserted into a
glass ampoule. The ampoule is placed in a desiccator which
contains phosphorus pentoxide (as drying agent) and which
is subsequently evacuated. The use of a vacuum is essential
because it reduces the time for which cells are exposed to the
deleterious effects of high concentrations of solute. When the
sample is completely desiccated the ampoule is sealed. Under
optimal conditions the organisms remain viable for years; spores
may remain viable for decades.
In general, desiccation is tolerated to different degrees by
different organisms; many do not survive for long in the airdried state. [Desiccation tolerance of prokaryotes: MR (1994)
58 755805.]
desmarestene See PHEROMONE.
Desmarestia See PHAEOPHYTA.
Desmidium A genus of placoderm DESMIDS.
desmids A group of freshwater, basically unicellular green
algae (division CHLOROPHYTA) which reproduce sexually by
conjugation and which never form flagellated cells of any kind.
In most species the cells are solitary, although in a few they are
joined end-to-end to form filaments (see e.g. HYALOTHECA). The
cells are generally more or less bilaterally symmetrical and may
be cylindrical, fusiform, crescent-shaped, etc, sometimes bearing
elaborate ornamentations. Many species are highly variable,
occurring in a range of growth forms a feature which has
caused considerable confusion in speciation and nomenclature
[Book ref. 123, pp. 251269].
In placoderm desmids each cell is divided into two semicells either by a median suture line (e.g. in Closterium and
Penium) or, more commonly, by an equatorial constriction
(sinus) the narrow region joining the semicells being called
the isthmus. The cell wall is perforated by pores through which
mucilage may be secreted; the mucilage may allow the desmid
to adhere to substrata, and is apparently necessary for the GLIDING MOTILITY often exhibited by these cells. Genera of placoderm desmids include e.g. CLOSTERIUM, COSMARIUM, Desmidium,
Euastrum, HYALOTHECA, Micrasterias, PENIUM, STAURASTRUM,
Staurodesmus, and XANTHIDIUM.
In saccoderm desmids the cells do not have a median
suture line or sinus and have smooth walls without pores.
They nevertheless produce mucilage, often in copious amounts,
and some can exhibit gliding motility. Genera include e.g.
Ancylonema (short cylindrical cells joined end-to-end to form
short filaments), Cylindrocystis (cells cylindrical, round-ended,
containing a stellate chloroplast at each end), and Mesotaenium
(cells short, cylindrical, solitary, containing a single chloroplast).
Sexual reproduction in desmids involves a process of conjugation analogous to that in SPIROGYRA. Essentially, cells come
Desulfococcus
Desulfovibrio
BACTERIA
230
DGGE
deuterosome In a eukaryotic cell: a dense region in the cytoplasm which can act as a MICROTUBULE-ORGANIZING CENTRE for
the de novo assembly of a BASAL BODY.
deutomerite In a cephaline gregarine: the posterior of the two
main regions of the (septate) cell (cf. PROTOMERITE); it usually
contains the nucleus.
DEV Duck embryo vaccine (see RABIES).
Devardas alloy An alloy containing aluminium (45%), copper
(50%) and zinc (5%); it is used e.g. to reduce nitrite and/or
nitrate to ammonia.
devils grip Syn. BORNHOLM DISEASE.
dew retting See RETTING.
dexioplectic metachrony See METACHRONAL WAVES.
dextrans D-Glucans in which the glucose residues are linked
mainly by (1 6)-a-glucosidic bonds; branches are formed by
occasional (1 4)-a- and, less frequently, (1 3)-a-linkages.
The size of the molecule and the nature and extent of branching
depend on the source of the dextran. Extracellular dextrans are
produced by a range of microorganisms, sometimes in copious
amounts (see e.g. ROPINESS); they are obtained commercially
from strains of Leuconostoc mesenteroides grown anaerobically
on sucrose-containing media [Book ref. 62, pp. 144]. Dextrans
of MWt ca. 75000 are used as plasma volume extenders for
blood transfusions; they may be obtained by acid hydrolysis
of higher-MWt dextrans. Artificially cross-linked dextrans (e.g.
Sephadex) are used in GEL FILTRATION. Dextrans are relatively
inert and can withstand autoclaving.
dextrins Products of the partial degradation of STARCH or GLYCOGEN by heat, acid hydrolysis, or enzyme action. Limit dextrins
are those formed by enzymes that are unable to effect complete
hydrolysis (see AMYLASES). (See also SCHARDINGER DEXTRINS.)
dextrose Dextrorotatory glucose (D-glucose).
DFD meat Dark, firm, dry meat: red meat from animals stressed
before slaughter. DFD meat contains less glucose and has a
higher pH (>ca. 6.0) than normal meat; during stress, muscle
glycogen in the living animal is converted to lactic acid (cf.
MEAT SPOILAGE) which is subsequently lost when the animal
is bled. DFD meat is more susceptible than normal meat to
spoilage. Increased susceptibility to aerobic spoilage appears
to be due to the deficiency of glucose rather than to the high
pH; since little or no glucose is available, spoilage organisms
attack amino acids earlier than in normal meat and, hence,
produce off-odours and off-flavours after a shorter period of
storage [Book ref. 30, pp. 240244]. Anaerobic spoilage (e.g.
in vacuum packs) may be due to organisms (e.g. Alteromonas
putrefaciens, Serratia liquefaciens) which are inhibited by the
low pH of normal meat. S. liquefaciens produces off-odours.
A. putrefaciens forms H2 S which reacts with e.g. myoglobin to
produce a green compound: sulphmyoglobin (greening) cf.
MEAT SPOILAGE (b); since A putrefaciens is inhibited at pH below
6.0, greening can be prevented by treating the meat with citrate
buffer. Vacuum-packed DFD meat may also support the growth
of large populations of Yersinia enterocolitica, although these
seem not to cause significant spoilage (cf. FOOD POISONING).
DFMO (DL-a-difluoromethylornithine) See SLEEPING SICKNESS.
DFP Diisopropylfluorophosphate see PROTEASES.
DGGE Denaturing gradient gel electrophoresis: a method for
comparing samples of related double-stranded DNA (generated
e.g. by PCR or restriction) by two-dimensional electrophoresis
(cf. SSCP). In DGGE [Biotechnology (1995) 13 137139], fragments are separated by size in the first phase of electrophoresis.
Then, in the same gel, the fragments are moved electrophoretically at right-angles to their original path. In this second phase,
DHBG
fragments move through an increasing concentration of DNAdenaturing agents (e.g. formamide + urea) so that, at certain
levels in the gradient, localized sequence-dependent melting
(i.e. strand separation) occurs within part(s) of the fragments
(base-pairing being stronger in GC-rich sections); such localized
melting affects the electrophoretic speed of those fragments in
which it occurs and allows separation of fragments in the gel.
[Example of use of DGGE (differentiation of isolates of
Escherichia coli by analysis of the 16S23S intergenic spacer
region): FEMS Ecol. (2001) 35 313321.]
Other uses of DGGE include e.g. characterization of organisms by comparing PCR-amplified sequences of their 16S rRNA
genes [AEM (1996) 62 340346] and detection of Rhizobium
spp [LAM (1999) 28 137141].
Another method, based on the same principle, replaces the
chemical denaturing gradient of DGGE with an ongoing increase
in temperature during the second phase of electrophoresis; thus,
at certain levels of temperature, localized sequence-dependent
melting occurs in specific part(s) of the fragments affecting
electrophoretic mobility and allowing separation within the gel.
This method is referred to as temporal temperature gradient gel
electrophoresis (TTGE).
[Comparison of DGGE with TTGE: LAM (2000) 30 427
431.]
DHBG (9-(3,4-dihydroxybutyl)-guanine) An ANTIVIRAL AGENT
which is active, both in cell cultures and in vivo, against herpes
simplex viruses (HSV-1 and -2); the (R)-enantiomer is more
effective than the (S )-enantiomer. The mechanism of action
resembles that of ACYCLOVIR, but DHBG has higher affinity for
HSV thymidine kinase.
DHBV DUCK HEPATITIS B VIRUS.
Dhori virus An unclassified virus (see ORTHOMYXOVIRIDAE)
which has been isolated from ticks; antibodies to the virus have
been found in man and domestic animals.
DHPA ((S )-DHPA; (S )-9-(2,3-dihydroxypropyl)-adenine) An ANTIVIRAL AGENT which acts as an analogue of adenosine; it is a
potent inhibitor of 5-adenosyl homocysteine hydrolase. DHPA is
active e.g. against vaccinia, herpes simplex, varicella-zoster and
measles viruses; it acts synergistically with VIDARABINE. (The
(R)-enantiomer is inactive.)
DHPG (9-(1,3-dihydroxy-2-propoxymethyl)-guanine; 2 -nor-2 -deoxyguanosine, 2 -NDG) An ANTIVIRAL AGENT which has potent
activity against herpes simplex viruses (HSV-1 and -2); it is not
effective against e.g. EpsteinBarr virus, varicella-zoster virus or
cytomegaloviruses. The mechanism of action resembles that of
ACYCLOVIR. The isomer (S )-9-(2,3-dihydroxy-1-propoxymethyl)guanine is also active against HSV-1 and -2.
DI particle DEFECTIVE INTERFERING PARTICLE.
diacetoxyscirpenol See TRICHOTHECENES.
diacetyl (dimethylglyoxal; CH3 .CO.CO.CH3 ) A water-soluble
compound formed e.g. by certain lactic acid bacteria; it may
also be derived by oxidation of acetoin in the BUTANEDIOL FERMENTATION. (See also VOGESPROSKAUER TEST.)
Diacetyl produced by certain lactic acid bacteria is responsible for the characteristic buttery flavour and aroma in many
fermented DAIRY PRODUCTS. The diacetyl is formed from pyruvate see Appendix III(c) but levels of diacetyl are low if the
pyruvate is derived from hexoses only. Additional pyruvate (and
hence diacetyl) can be produced from citrate by certain strains of
lactic acid bacteria (aroma bacteria, flavour bacteria) e.g.
Lactococcus lactis and Leuconostoc cremoris (see LACTIC ACID
STARTERS). (Citrate is naturally present in cows milk at levels
of ca. 0.2%, with seasonal fluctuations; it may also be added to
diatoms
etc which are usually arranged in symmetrical, species-specific
patterns. The degree of cell wall silicification may vary to
some extent with environmental conditions, and exceptionally
the wall may be predominantly or entirely organic (e.g. in Phaeodactylum tricornutum see PHAEODACTYLUM and in Cylindrotheca fusiformis). [Details of wall structure: Book ref. 137,
pp. 129156.]
Two main groups of diatoms are commonly recognized:
centric diatoms, in which the valve is radially symmetrical, and
pennate diatoms, in which the valve is bilaterally symmetrical.
(Some diatoms do not fit easily into either category: e.g.
Triceratium spp may have 3-, 4- or 5-fold rotational symmetry;
see also HEMIDISCUS.)
Centric diatoms are mostly marine and planktonic, are nonmotile, and commonly exhibit oogamous sexual reproduction
in which the male gametes each bear a single tinsel flagellum. Genera include e.g. Arachnoidiscus, Bacteriastrum, Biddulphia, CHAETOCEROS, Coscinodiscus, Cyclotella, Hemiaulus,
MELOSIRA, Skeletonema, Stephanodiscus, Stephanopyxis, Thalassiosira, Zygoceros.
Pennate diatoms occur in various habitats; many are capable of
gliding motility, and many exhibit isogamous sexual reproduction involving cellcell contact (conjugation). All species which
are capable of GLIDING MOTILITY (q.v.) have a raphe: basically,
a slit which (usually) runs the length of the valve, interrupted
by a central nodule. Such raphid species are generally benthic or occur attached to a solid substratum. In a few genera
(e.g. Achnanthes, Cocconeis) a raphe occurs in only one of the
two valves, but in most a raphe occurs in both valves. Pennate diatoms which lack a raphe (araphid diatoms: e.g. Fragilaria, Striatella, Tabellaria) cannot glide; these organisms may
have a central line, ridge, or unornamented central area called
a pseudoraphe. (Other pennate diatoms include e.g. AMPHORA,
Anomoeoneis, Bacillaria, Cylindrotheca, Cymbella, Diatoma,
GOMPHONEMA, Gyrosigma, NAVICULA, Nitzschia, PHAEODACTYLUM, Pinnularia, Pleurosigma, Stauroneis, Surirella.)
In many centric and pennate diatoms the cells adhere to one
another to form filaments or characteristic groupings (see e.g.
ASTERIONELLA and MELOSIRA); the cells may be held together by
mucilage secreted via tubular projections in the frustule and/or
by the interlocking of spines present on the margins of the
valves. Secreted mucilage may also serve to attach some forms
to the substratum, and apparently serves an essential role in
GLIDING MOTILITY.
Asexual reproduction occurs by binary fission. The nucleus
(which is diploid in vegetative cells) moves from its position
near the epivalve to the cell centre, and the protoplast expands,
pushing the two valves apart. New girdle bands are formed,
and mitosis occurs. The original parent hypovalve becomes
the epivalve of one daughter cell, and both daughter cells
synthesize a new hypovalve. Thus, the epivalve is always the
older of the two valves in a cell, and in species in which
the epivalve is larger than the hypovalve one of the daughter
cells must be smaller than the parent cell. When division is
complete, the nucleus in each cell returns to its position near
the epivalve face. The new siliceous structures (valves and
cingulum) are synthesized in SILICA DEPOSITION VESICLES beneath
the plasmalemma, reaching the exterior by fusion between the
silicalemma and plasmalemma. [Diatom wall formation: Book
ref. 137, pp. 157200; silicon biomineral synthesis in diatoms:
TIBS (1987) 12 151154.]
Since, in many species, the average size of cells in a
population progressively decreases with increasing numbers of
diatoxanthin
Dick test A SKIN TEST used to determine whether or not an
individual is susceptible to SCARLET FEVER. The test procedure
(similar to that used in the SCHICK TEST) involves an intradermal
injection of the erythrogenic toxin of Streptococcus pyogenes.
A positive Dick test (indicating susceptibility) consists of an
inflammatory response (at the site of the injection) which
becomes evident within ca. 12 hours and reaches peak intensity
within ca. 24 hours of the injection. In immune individuals the
toxin is neutralized by antitoxin, thus giving a negative test.
dicloran An agricultural antifungal agent (2,6-dichloro-4nitroaniline) which is used against various Botrytis infections.
It is water-insoluble hence very persistent and is usually
formulated as a dust; it has very low phytotoxicity. (cf.
CHLORONITROBENZENES.)
dicloxacillin See PENICILLINS.
Dictyocha See SILICOFLAGELLATES.
Dictyoglomus A genus of bacteria. One species: D. thermophilum,
an anaerobic, caldoactive, asporogenous chemoorganotroph;
cells: rod-shaped, occurring in large spherical bodies consisting
of a few to many separate cells. [IJSB (1985) 35 253259.]
Dictyosiphon See PHAEOPHYTA.
dictyosome (1) One of the stacks of membranous vesicles which
form a GOLGI APPARATUS. (2) Syn. Golgi apparatus.
dictyosporae See SACCARDOAN SYSTEM.
Dictyostelia See EUMYCETOZOEA.
dictyostelids See DICTYOSTELIOMYCETES.
Dictyosteliia See EUMYCETOZOEA.
Dictyosteliomycetes (dictyostelid cellular slime moulds; dictyostelids) A class of cellular SLIME MOULDS (division MYXOMYCOTA). (cf. EUMYCETOZOEA.) The organisms occur mainly in soil,
humus and dung, particularly in tropical regions. The vegetative phase consists of myxamoebae which form filose subpseudopodia; flagellated cells are not formed. The life cycle
involves a feeding stage, during which myxamoebae ingest
food (mainly bacteria) and divide mitotically. When the food
supply is exhausted, the amoebae stop growing and, after a
period of starvation (pre-aggregation phase or interphase),
the aggregation phase begins: numerous myxamoebae converge
(chemotactically see ACRASIN) and join together to form one
to many multicellular, macroscopic pseudoplasmodia. In most
species, the pseudoplasmodium can migrate over the surface of
the substratum and can show tactic responses. Eventually, the
pseudoplasmodium stops moving and differentiates to form a
multicellular, multispored, stalked fruiting body, the sorocarp
(a process known as culmination); the sorocarp stalk consists
of a cellulosic stalk tube which, when mature, is either hollow or filled with dead cells. The spores are dispersed by
wind, rain, etc; on germination, each spore releases a myxamoeba, thus initiating a new cycle. (In some species myxamoebae
may not always pass through this life cycle, forming instead
MICROCYSTS and/or MACROCYSTS.) Genera: e.g. ACYTOSTELIUM,
DICTYOSTELIUM, POLYSPHONDYLIUM.
[Dictyostelids natural history, life cycles, cultivation: Book
ref. 144.]
Dictyostelium
A genus of slime moulds (class DICTYOSTELIOMYCETES) in which the sorocarp stalk tube is filled with a
mesh of empty cell walls (cf. ACYTOSTELIUM) and bears a spherical sorus of spores at its apex. In e.g. D. discoideum the sorocarp
consists of a single unbranched stalk that tapers from base to tip;
the proximal end is flared into a basal attachment disc, and the
distal end bears a single, more or less spherical, white to yellowish mass (sorus) of ellipsoidal to reniform spores (each typically
ca. 2.53.5 6.09.0 m). In some species the sorocarp may
Didinium
substratum, exhibiting e.g. aerotaxis, phototaxis and thermotaxis.
The slime sheath does not move relative to the substratum, and
may provide traction against which the cells within can move;
thus, as the slug moves forwards, a slime trail of collapsed sheath
material remains behind. New sheath material is synthesized
along the length of the slug, so that the sheath is thinnest at
the anterior end, becoming progressively thicker towards the
posterior. A migrating slug can split into two smaller slugs, or
two slugs can merge to form a larger slug; the size (but not the
proportions) of the sorocarp which eventually develops depends
on the size of the slug at culmination.
The fates of the cells during culmination are apparently determined at the slug migration stage (i.e., before culmination
begins): the cells making up the anterior third of the slug are
prestalk cells, destined to form the sorocarp stalk, while the
cells of the posterior two-thirds are prespore cells. [Patterns of
cell differentiation within the slug: Book ref. 67, pp. 255274.]
The culmination process begins when the slug stops moving and
reorientates such that the leading (anterior) tip is raised vertically
above the rest of the cell mass, forming a nipple-like apical projection. A short cellulosic stalk tube initial is secreted by cells
near the apex; the entire cell mass then flattens, bringing the
tube down through the cell mass to the substratum. Prestalk cells
within the lower end of the tube enlarge, become vacuolated and
compacted, and eventually die; the stalk lengthens upwards the
remaining prestalk cells progressively undergoing vacuolation
and death to result eventually in the characteristic mesh of cellulose cell walls which fills the cellulose stalk tube. Meanwhile,
the mass of prespore cells is gradually elevated on the growing
stalk, becoming progressively differentiated into spores from the
periphery to the centre of the mass. Differentiation is complete
when all the cells have become either stalk cells or spores.
The sorocarp is usually orientated such that the sorus is at
the maximum distance from the substratum or from adjacent
objects (including other sorocarps); this orientation is believed
to be due to a tropism regulated by an (unidentified) gas or
vapour produced by the developing sorocarp.
The spores have thick cellulosic walls and are resistant to e.g.
desiccation. Germination generally occurs only in the presence
of an adequate supply of amino acids. Spores in masses fail to
germinate owing to the presence of an autoinhibitor apparently
produced during culmination.
In D. discoideum macrocysts may be formed, but microcysts
have not been observed.
Dictyota See PHAEOPHYTA.
Dictyuchus See SAPROLEGNIALES.
dicyandiamide (DCD; Didin) Cyanoguanidine, a NITRIFICATION
INHIBITOR. [Mineralization of DCD in acid soils: SBB (1985) 17
253254.]
N,N -dicyclohexylcarbodiimide See DCCD.
didanosine See NUCLEOSIDE REVERSE TRANSCRIPTASE INHIBITORS.
didemnins Cyclic depsipeptide ANTIVIRAL AGENTS isolated from
Caribbean tunicates (sea-squirts); they are probably too cytotoxic
for therapeutic use.
dideoxy fingerprinting See TUBERCULOSIS (antibiotic resistance
testing).
dideoxy sequencing See DNA SEQUENCING.
dideoxyribonucleotide See NUCLEOTIDE (figure legend).
dideoxythymidine triphosphate See DDTTP.
Didesmis See GYMNOSTOMATIA.
Didin See DICYANDIAMIDE.
Didinium A genus of freshwater ciliates (subclass GYMNOSTOMATIA). Cells: radially symmetrical, ovoid or barrel-shaped, ca.
Didymella
site, the 3 -AAA . . . tail on polyadenylated mRNA molecules.
The task is made manageable by converting only some of the
(many) mRNAs from each population; selectivity is achieved
with a primer such as 5 -TT . . . TTGG-3 which permits conversion of only those mRNAs in which a cytosine (C) residue
occurs in the appropriate position after the 3 -AAA . . . tail.
cDNAs from each of the populations are then fingerprinted by
subjecting them to ARBITRARILY PRIMED PCR and separating the
products by gel electrophoresis. When fingerprints from different
populations are compared, any band(s) of interest such as
band(s) present in one fingerprint but not in other(s) can be
further examined by removal from the gel and amplification by
the same arbitrary primer; the amplified fragments may be e.g.
sequenced and/or used to probe a library.
[Differential display methodology: NAR (1998) 26 5537
5543; review: Biotechniques (2002) 33 338346.]
differential host (plant pathol.) A plant host which, on the basis
of disease symptoms, serves to distinguish between various
strains or races of a given plant pathogen.
differential interference-contrast microscopy See MICROSCOPY (d).
differential medium See MEDIUM.
diffluent Readily dissolving or breaking up in water.
Difflugia A genus of testate amoebae (order ARCELLINIDA) in
which the test is reinforced with sand grains, diatom frustules,
sponge spicules etc which are initially ingested by the cell.
D. urceolata is multinucleate and has a rounded test (ca.
200230 150200 m) with a pointed top and a rim around
the ventral aperture through which several narrow, round-ended
pseudopodia emerge. Difflugia spp occur in ponds, swamps,
bogs, soil etc.
diffusely adherent E. coli See ENTEROADHERENT E. COLI.
diffusion-coupled gradostat See GRADOSTAT.
diffusion test (1) In ANTIBIOTIC-sensitivity testing: any test which
involves the diffusion of antibiotic(s) through agar. See e.g. DISC
DIFFUSION TEST and AGAR DIFFUSION TEST.
(2) (for membrane filters) A test used to determine the physical
integrity of a membrane filter (see FILTRATION). If a wetted
membrane is subjected to a pressure lower than its bubble point
pressure (see BUBBLE POINT TEST), some air can pass through the
pores by simple diffusion; the amount of air transmitted in this
way can be significant in filters of large surface area. In the
diffusion test a wetted filter is subjected to pressure at ca. 80%
of its bubble point pressure, and the volume of air transmitted is
determined; the integrity of the filter is assessed by comparing
this volume with that expected from an intact filter.
DL-a-difluoromethylornithine See SLEEPING SICKNESS.
difolatan Syn. CAPTAFOL.
DIG Abbreviation for DIGOXIGENIN.
digenetic Refers to a parasite which carries out part of its life
cycle in each of two different host species. (cf. HETEROXENOUS.)
di George syndrome (congenital thymic aplasia) The condition,
resulting from an undeveloped thymus gland, which is characterized by a lack of T LYMPHOCYTES; those with this syndrome
are susceptible to a range of infections, especially by intracellular pathogens. The condition has been treated by transplantation
of fetal thymus gland (using tissue from a fetus at <14 weeks
gestation).
digitonin A mixture of steroid SAPONINS found in the seeds of
the purple foxglove (Digitalis purpurea).
digoxigenin (DIG) A (poisonous) steroid obtained from species
of the plant Digitalis. Digoxigenin is used e.g. as a tag for
non-radioactive labelling of oligonucleotide probes (both RNA
and DNA) see e.g. DOT-BLOT.
dimixis
than those with lower coefficients e.g. chlorhexidine (h = 2),
QACs (h = 1).
dilution end-point assay See END-POINT DILUTION ASSAY.
dilution rate (D) In CONTINUOUS CULTURE: the parameter F/V in
which F is the rate at which medium enters (and leaves) the
culture vessel, and V is the volume of liquid in the vessel.
Dilution rate has the same dimensions as SPECIFIC GROWTH RATE
(i.e., 1/time) and its unit is hour1 . Under steady-state conditions
dilution rate is numerically equal to specific growth rate. The
critical dilution rate (Dc ) is the dilution rate which corresponds
to mmax ; if the dilution rate exceeds Dc the culture is eventually
diluted to extinction and is said to have undergone wash-out.
dilution test In ANTIBIOTIC-sensitivity testing: a procedure in
which an organism is tested for its ability to grow in the
presence of certain fixed concentrations of a given antibiotic.
(cf. DIFFUSION TEST.)
In the agar dilution test (= plate dilution test) a series of agar
plates containing progressively lower concentrations of a given
antibiotic (and an antibiotic-free control plate) are each surfaceinoculated with the test organism and incubated; the MIC (q.v.)
is indicated by the lowest concentration of antibiotic at which
growth does not occur.
The broth dilution test (= tube dilution test) is essentially
similar (in principle and interpretation) to the agar dilution test
except that growth of the test organism is attempted in each of a
series of broths containing progressively lower concentrations of
antibiotic. If each broth is ca. 0.2 ml or less the process may be
called a microdilution broth test; otherwise it is a macrodilution
broth test.
Dimargaritales See ZYGOMYCETES.
Dimastigamoeba gruberi A former name of Naegleria gruberi.
dimension (1) (serol.) In GEL DIFFUSION procedures: the mode
in which antibody and antigen come together in order to form
precipitate. In single dimension tests, antigen and/or antibody
diffuse through the gel in a single direction i.e., parallel to the
long axis of a gel column. In double dimension tests, a given
reactant (antigen and/or antibody) diffuses radially outwards
from a hole or well cut into the gel. (See also SINGLE DIFFUSION
and DOUBLE DIFFUSION.)
(2) Either stage of TWO-DIMENSIONAL ELECTROPHORESIS.
Dimerella See GYALECTALES.
dimethirimol (5-n-butyl-2-dimethylamino-4-hydroxy-6-methylpyrimidine) A HYDROXYPYRIMIDINE ANTIFUNGAL AGENT which is
active against powdery mildews of chrysanthemums, cucurbits
and sugar beet.
dimethyldithiocarbamate See DMDC.
dimethylglyoxal Syn. DIACETYL.
dimethyloxazolidinedione (DMO) See CHEMIOSMOSIS.
dimethylsulphoxide (DMSO; (CH3 )2 SO) A non-ionized polar
solvent used e.g. as a cryoprotectant in FREEZING. Both
hydrophilic and lipophilic substances are soluble in DMSO.
dimetridazole (Emtryl) 1,2-Dimethyl-5-nitro-imidazole: a NITROIMIDAZOLE antimicrobial agent used in veterinary medicine e.g.
for the prevention and treatment of BLACKHEAD in turkeys and
of SWINE DYSENTERY.
dimictic Of, or pertaining to, DIMIXIS.
dimidiate (1) Split into two. (2) Lacking or appearing to
lack one half (applied e.g. to a semicircular, non-stipitate
fungal fruiting body).
dimitic See HYPHA.
dimixis (1) Morphological HETEROTHALLISM. (2) One-locus twoallele physiological heterothallism.
dimorphic fungi
perpendicularly from the girdle into the hypocone. One of the
two flagella (the transverse flagellum) lies in the girdle and
encircles the cell, while the other (longitudinal ) flagellum arises
from the sulcus and may project beyond the cell. The transverse
flagellum [form and function: JP (1985) 32 290296] is longer
than the longitudinal one, is helical in shape, contains a PARAXIAL
ROD, and bears a single row of fine hairs; the longitudinal
flagellum may be smooth or may bear two rows of stiffer hairs.
(cf. e.g. PROROCENTRUM; see also PUSULE.) Dinoflagellate cells
contain contractile, non-actin filaments which are apparently
responsible for cell contraction and shape changes in at least
some species (Kofoidinium and related genera [Cell Mot. (1985)
5 115]).
The dinoflagellate nucleus contains chromosomes which are
unique among eukaryote chromosomes in lacking centromeres
and containing little or no protein; dinoflagellate nuclear organization has been considered to be intermediate between prokaryotic and eukaryotic, and has been termed mesokaryotic or
dinokaryotic. During MITOSIS the nuclear membrane remains
intact; the spindle is typically extranuclear spindle MTs passing through the nucleus via channels lined with nuclear membrane but in Oxyrrhis marina the spindle is wholly intranuclear [JCS (1986) 85 161175].
The majority of dinoflagellates are photosynthetic, typically
possessing several chloroplasts per cell and containing chlorophylls a and c2 , b-carotene, and peridinin (replaced by fucoxanthin in Glenodinium foliaceum). Other dinoflagellates (e.g.
NOCTILUCA) are colourless and heterotrophic. Both heterotrophic
and photosynthetic species can apparently ingest particulate matter in the region of the sulcus.
Resistant resting spores (cysts, hypnospores) are produced
in some species. [Cyst formation in Gonyaulax tamarensis:
JEMBE (1985) 86 113.] (cf. HYSTRICHOSPHAERIDS.) Sexual
reproduction has been observed in some species.
The majority of dinoflagellates are free-living in marine,
brackish or freshwater habitats, sometimes forming extensive
blooms (see e.g. RED TIDE). Some dinoflagellates (e.g. species of
Gonyaulax, Noctiluca, Pyrocystis, Pyrodinium) exhibit BIOLUMINESCENCE, and some produce potent toxins (see e.g. SAXITOXIN).
Dinoflagellates also occur in association with other organisms:
e.g. Blastodinium is parasitic in the intestines of copepods,
Oodinium is a parasite of fish (see VELVET DISEASE), and Symbiodinium is an endosymbiont in various invertebrates (see
ZOOXANTHELLAE).
Dinoflagellida See PHYTOMASTIGOPHOREA.
dinokaryotic See DINOFLAGELLATES.
Dinophyceae See DINOFLAGELLATES.
Dinothrix A genus of marine DINOFLAGELLATES in which the
cells are non-motile and are joined together to form branching
filaments.
Diodoquin See 8-HYDROXYQUINOLINE.
dioecious Refers to an organism in which the male and female
reproductive structures occur in different individuals. (cf. MONOECIOUS.)
dioecism Morphological HETEROTHALLISM.
1,2-dioxetane A type of substrate which gives rise to CHEMILUMINESCENCE when activated by certain enzymes (examples: AMPPD
and CSPD).
dioxygenase See OXYGENASE.
dip-slide method (agar-slide method) A method for detecting or
estimating microbial populations on solid surfaces and in various
fluids (e.g. machine-tool cooling fluids, urine samples). The dipslide, a plastic slide coated with a sterile nutrient agar, is attached
dimorphic fungi (1) Those fungi (e.g. species of Blastomyces and Candida) which according to environmental conditions can grow in either of two distinct vegetative states: a
unicellular (yeast-phase) state or a mycelial state. (See GROWTH
(fungal); MORPH.) (See also QUORUM SENSING.)
(2) Fungi which exhibit DIPLANETISM.
(3) Syn. DIOECIOUS fungi.
din genes In Escherichia coli, DNA damage-inducible genes:
genes inducible in the SOS SYSTEM. For dinB see DNA POLYMERASE IV.
dinactin See MACROTETRALIDES.
dinitrogen fixation Syn. NITROGEN FIXATION.
dinitrogenase Syn. NITROGENASE.
2,4-dinitrophenol See PROTON TRANSLOCATORS.
dinitrophenols Dinitrophenols exhibit antifungal, insecticidal
and herbicidal properties. As ANTIFUNGAL AGENTS they are used
mainly for the treatment of powdery mildews; they include
binapacryl (2,4-dinitro-6-sec-butyl-phenyl-3-methylcrotonate),
which is also an acaricide, dinobuton (2,4-dinitro-6-sec-butylphenylisopropylcarbonate), and dinocap (a mixture of three
isomers of each of the compounds 2,4-dinitro-6-sec-octylphenol
and 2,6-dinitro-4-sec-octylphenol in which the octyl group may
be 1-methylheptyl, 1-ethylhexyl or 1-propylpentyl). Dinocap is
generally used as the crotonate; it functions as an antifungal
ERADICANT and PROTECTANT. (See also PROTON TRANSLOCATORS.)
Dinobryon
A genus of loricate, generally colonial CHRYSOPHYTES. Each cell has two flagella of unequal length, and sits
in a stalked, vase-shaped LORICA composed of helical bands of
cellulose microfibrils which are laid down by the slowly rotating
cell within. Following cell division, one daughter cell becomes
attached to the rim of the parent lorica and secretes a new lorica
around itself, so that eventually a branching, fan-shaped colony
is formed.
dinobuton See DINITROPHENOLS.
dinocap See DINITROPHENOLS.
dinoflagellates A large group of photosynthetic and/or heterotrophic organisms regarded either as algae (e.g. class Dinophyceae, division Dinophyta) or as protozoa (see PHYTOMASTIGOPHOREA). Most dinoflagellates are unicellular and biflagellated (but cf. e.g. CYSTODINIUM, DINOTHRIX and GLOEODINIUM).
The cell typically has a theca composed essentially of a layer of
flattened membranous vesicles beneath the plasmalemma; these
vesicles may be empty (in unarmoured dinoflagellates such as
Gymnodinium, Gyrodinium, and Oxyrrhis) or may each contain
a cellulosic plate varying from very thin (e.g. in Katodinium
and Woloszynskia) to thick (in armoured dinoflagellates such
as Ceratium and Peridinium). The edges of thick plates are commonly bevelled, allowing the plates to move freely relative to
each other. The number of plates per cell ranges from two (e.g.
in PROROCENTRUM) to several hundred, the number, form and
arrangement of plates being characteristic for a given dinoflagellate. (See also e.g. CERATIUM; ORNITHOCERCUS.) On cell division,
the thecal plates may be shared between the daughter cells, each
cell then synthesizing new plates to replace those taken by the
other; in e.g. Gonyaulax shedding of the theca (ecdysis) by the
parent cell occurs prior to cell division.
In the majority of dinoflagellates (including e.g. Amphidinium,
Ceratium, Glenodinium, Gonyaulax, Gymnodinium, Oxyrrhis,
Peridinium and Woloszynskia) the vegetative cell is divided by
a transverse groove (the girdle, cingulum or annulus) into two
parts: the epicone and the hypocone. (The corresponding thecal
regions in armoured dinoflagellates are termed the epitheca
and hypotheca.) A longitudinal groove, the sulcus, extends
238
diplococcus
to the inside of the cap in a screwcap cylindrical tube; for use,
the cap is unscrewed and the slide is dipped into, or pressed
against, the sample and it is subsequently incubated. Microbial
numbers can be estimated from the number of colonies which
develop on the slide. (See also COUNTING METHODS.)
diphasic medium Any MEDIUM, e.g. NNN MEDIUM, in which a
solid (usually agar-based) component is at least partly covered
by a liquid overlay.
diphasic serotypes See H ANTIGEN (Salmonella).
diphenyliodonium chloride See IODONIUM COMPOUNDS.
diphenylthiourea See THIOUREA DERIVATIVES.
diphenylurea See CARBANILIDES.
diphosphopyridine nucleotide See NAD.
diphthamide See DIPHTHERIA TOXIN.
diphtheria (membranous croup) An acute infectious human disease, usually affecting children, caused by toxinogenic strains of
Corynebacterium diphtheriae. Infection occurs by droplet inhalation or ingestion of contaminated food, milk etc. Asymptomatic
carriers are often sources of infection. Incubation period: 110
(usually 25) days. Symptoms: fever, sore throat, headache, and
the development of a characteristic whitish or grey membrane
at the site of infection usually the tonsils but sometimes e.g.
the nasopharynx, larynx, or nose; the membrane and swelling
of adjacent tissues can cause respiratory obstruction and difficulty in swallowing. Other sites occasionally affected include
skin lesions or wounds (cutaneous diphtheria) and the genitals.
The membrane results from the local effects of the DIPHTHERIA
TOXIN which causes cell death and subsequent deposition of fibrin, blood cells, cellular debris, and C. diphtheriae cells. Local
secondary infection with e.g. Streptococcus pyogenes (septic
diphtheria) may occur. C. diphtheriae normally remains localized at the membrane, but the toxin is disseminated via the
blood and lymph and can cause severe, often fatal, systemic
effects including myocarditis and nerve demyelination. Treatment : primarily with antitoxin. Penicillin G or erythromycin
may be used in treatment and for eradication of C. diphtheriae from carriers. Lab. diagnosis: culture of C. diphtheriae (see
CORYNEBACTERIUM) from swabs, and/or identification of the toxin
(e.g. by gel diffusion tests).
[Review: RMM (1996) 7 3142.]
diphtheria toxin A heat-labile protein exotoxin (MWt ca. 60000)
produced by certain lysogenic strains of Corynebacterium diphtheriae and responsible for the symptoms of DIPHTHERIA; it is
lethal for many animal species and is also cytotoxic in some
types of cell culture e.g. Vero cells are highly susceptible,
though murine cells are almost totally resistant. (cf. EXOTOXIN A.)
Diphtheria toxin (DT) is encoded by tox, a gene carried by various temperate CORYNEPHAGES (e.g. b, !, g) [tox + corynephages
(DNA relationships): Inf. Immun. (1985) 49 679684].
The toxin is synthesized as a single polypeptide chain. The Yshaped molecule consists of three domains: translocation domain,
receptor-binding domain (RBD) and catalytic domain (CD).
Uptake of toxin involves initial binding of the RBD to a
receptor protein, and internalization of the toxin within a vesicle
via a clathrin-coated pit (PINOCYTOSIS). In the vesicle, CD is
proteolytically cleaved but remains attached via a disulphide
bond; the translocation domain undergoes an acid-induced
conformational change in which it inserts into the membrane
of the vesicle apparently forming a pore through which CD is
translocated into the cytoplasm of the target cell. The disulphide
link undergoes reduction (scission) releasing CD into the
target cells cytoplasm.
CD is a heat-stable fragment with resistance to cellular proteolysis. It has ADP-ribosyltransferase activity, and, in the cell,
Diplococcus pneumoniae
Diplococcus pneumoniae
Incorrect name for Streptococcus
pneumoniae.
Diplodia See SPHAEROPSIDALES.
Diplodinium
A genus of ciliates (order ENTODINIOMORPHIDA)
which occur e.g. in the RUMEN. The cytostome is close to
the anterior pole of the cell; somatic ciliature is limited, cilia
occurring in tufts in the oral and anteriodorsal regions. (See also
DZM.) The pellicle may be drawn out posteriorly into one or
more spines.
Diploicia A genus of placodioid LICHENS (order LECANORALES).
Apothecia: lecideine, black; ascospores: brown, one-septate.
D. canescens (formerly Buellia canescens) has a whitish thallus
bearing whitish-grey farinose soralia; this species is common
in Atlantic regions of Europe, growing on rocks, wood, bark
etc. particularly in light shade.
diploid Having a PLOIDY of two. (cf. HAPLOID and POLYPLOID.) In
a prokaryotic cell, partial diploid or merodiploid refers to the
possession of extra copies of only some of the chromosomal
genes see MEROZYGOTE.
Diplomastigomycotina See OOMYCETES.
Diplomonadida An order of protozoa (class ZOOMASTIGOPHOREA); cells contain either one (suborder Enteromonadina)
or two (suborder Diplomonadina) KARYOMASTIGONTS, those
containing two exhibiting twofold rotational symmetry or (in
Giardia) bilateral symmetry. Each karyomastigont has 14
flagella. Mitochondria and Golgi apparatus are absent.
Members of the Enteromonadina are parasitic; cysts are
formed in at least one genus. Genera: e.g. Enteromonas, Trimitus.
In the Diplomonadina each karyomastigont has four flagella,
one of which is recurrent. Cysts are formed by at least some
species. The suborder includes free-living and parasitic species.
Genera: e.g. GIARDIA, HEXAMITA, Trepomonas.
Diplomonadina See DIPLOMONADIDA.
diplont (1) (noun) An organism in whose life cycle only the
gametes are haploid. (cf. HAPLONT.) (2) The diploid form of an
organism, e.g. a sporophyte (see ALTERNATION OF GENERATIONS).
(3) (diplontic) (adj.) Refers to either (1) or (2) above.
diplophage A bacteriophage which infects Streptococcus (Diplococcus) pneumoniae.
diplophase In organisms which reproduce sexually: the diploid
phase of the life cycle (between syngamy and MEIOSIS).
Diplornaviridae A family proposed for all dsRNA-containing
viruses; the family has not been accepted since differences in
genome structure, replication and expression among dsRNA
viruses are too great to be encompassed in a single family.
Diploschistes See GRAPHIDALES.
diplostichomonad membrane See PARORAL MEMBRANE.
diplotene stage See MEIOSIS.
Diplotheca See CHOANOFLAGELLIDA.
Dipodascaceae See ENDOMYCETALES.
Dipodascus
See ENDOMYCETALES and GEOTRICHUM; see also
AMBROSIA FUNGI.
dipyridine ferrohaemochrome See CYTOCHROMES.
direct epifluorescent filter technique See DEFT.
direct immunofluorescence See IMMUNOFLUORESCENCE.
direct repeat (DR) Either of two (or more) regions of a nucleic
acid molecule in which the sequences of bases or base pairs are
similar or identical and have the same polarity and orientation,
e.g.:
5 . . . GGCT . . . GGCT . . . 3
3 . . . CCGA . . . CCGA . . . 5
The repeated sequences may or may not be contiguous. (cf.
INVERTED REPEAT.)
240
DNA chip
of Z-DNA) and also the unwinding of DNA strands e.g. during DNA REPLICATION, RECOMBINATION, TRANSCRIPTION, etc. The
degree of supercoiling of DNA in vivo is controlled by enzymes
called TOPOISOMERASES.
Normal cellular function requires that the degree of supercoiling be maintained within certain limits. In some circumstances e.g. during the transition from aerobic growth to anaerobic growth there is a fall in the cells energy charge and a
corresponding, transient fall in global (i.e. overall) superhelical
density; such changes in superhelicity alter the expression of a
range of genes (e.g. by affecting the activity of their promoters).
Local increases in superhelicity (i.e. in specific regions of the
DNA molecule) can be brought about by divergent transcription
from closely spaced promoters; such increased negative superhelicity may affect the expression of particular genes/operons
[Mol. Microbiol. (2001) 39 11091115].
Pure linear dsDNA clearly cannot be supercoiled. However,
linear dsDNA (and discrete regions or domains within linear or
ccc dsDNA) can maintain a superhelical conformation if there
is a constraint on the rotation of the double helix to prevent
unwinding of the supercoils (see CHROMATIN and CHROMOSOME
(bacterial)).
Certain drugs exert their toxic effects by binding to DNA; the
drug may bind e.g. to the major or minor grooves of dsDNA (see
e.g. NETROPSIN) or may intercalate between the base-pairs (see
INTERCALATING AGENTS). [DNA structure and its perturbation by
drug binding (review): Bioch. J. (1987) 243 113.]
See also GC%; DNA HOMOLOGY; THERMAL MELTING PROFILE.
DNA I Supercoiled ds cccDNA (see DNA).
DNA I Syn. DNA IV (q.v.).
DNA II Nicked relaxed circular dsDNA formed by an ss nick
in DNA I.
DNA III Linear dsDNA derived from DNA I or DNA II by
strand breakage.
DNA IV (DNA I ) Relaxed (intact) ds cccDNA (see DNA).
DNA base composition See e.g. BASE RATIO and GC%. (See also
DNA HOMOLOGY.)
DNA binding protein (1) Syn. SINGLE-STRAND BINDING PROTEIN.
(2) In general: any non-enzymic protein which binds to ssDNA
or dsDNA e.g. a repressor protein, or a single-strand binding
protein.
DNA blotting See BLOTTING.
DNA chip A microarray of short, single-stranded DNA molecules having diverse (but known) sequences immobilized
on a small piece (chip) of glass, silicon or plastic. The
immobilized DNA molecules commonly function as PROBES. A
chip can be used e.g. to determine the sequence of an unknown,
labelled, single-stranded fragment of nucleic acid by testing the
ability of the fragment to hybridize with a particular probe
in the array, hybridization being detected by the fragments
label using e.g. confocal epifluorescence microscopy.
A large microarray of probes can cover all possible combinations of nucleotides for a strand of given length. For example, a
complete set (48 ) of nucleotide combinations for an 8-nucleotide
probe 65536 different probes can be synthesized on a 1 cm2
glass chip.
Chips are useful e.g. for detecting mutations, including those
that confer resistant to antibiotics. Thus, that section of a
genome in which mutations confer resistance to particular
antibiotic(s) can be amplified (e.g. by PCR using fluorophorelabelled primers), and the amplicons tested against a microarray
which includes all possible mutations (as well as the wildtype sequence). For example, the protease gene in clade B
DNA cloning
interpret. One solution to the problem is to use a rare-cutting
RE (see table in RESTRICTION ENDONUCLEASE); this gives fewer,
larger fragments that can be analysed e.g. by PFGE.
Alternatively, the original procedure can be carried out with
additional use of a labelled probe that reveals only those (few)
fragments to which the probe binds; an example of this approach
is RIBOTYPING (q.v.).
[Evidence from DNA fingerprinting of endoscopic crossinfection in post-endoscopic acute gastritis (Helicobacter pylori ):
JCM (2000) 38 23812382.]
(See also FINGERPRINTING.)
dna genes In Escherichia coli : those genes whose products are
involved in at least some types of DNA REPLICATION. See separate
entries for genes dnaA, dnaB, dnaC (= dnaD), nrdA (= dnaF),
dnaI, dnaJ, dnaK, dnaP and dnaT. For dnaE, dnaN, dnaQ,
dnaX and dnaZ (= dnaH) see DNA POLYMERASE. For dnaG see
PRIMASE. For dnaW see adk gene.
DNA glycosylase See ADAPTIVE RESPONSE and URACIL-DNA GLYCOSYLASE.
DNA gyrase Syn. GYRASE.
DNA helicases Syn. HELICASES.
DNA homology The degree of similarity (relatedness) between
base sequences in different DNA molecules (or in different parts
of the same DNA molecule); two DNA molecules which are
100% homologous have identical sequences of nucleotides.
In microbial TAXONOMY the degree of homology between
samples of chromosomal DNA from different organisms can
be used to indicate the taxonomic relationship of the organisms.
The homology between two samples of dsDNA can be assessed
by various indirect methods (as well as by sequencing each
sample and making a direct comparison of the nucleotides); two
approaches are outlined below.
In DNADNA hybridization, single-stranded (heat-denatured)
chromosomal DNA from one test strain (strain A) is bound
to a membrane (e.g. nitrocellulose). Chromosomal DNA from
another test strain (strain B) is fragmented (for example, by
ULTRASONICATION) and the fragments denatured by heat to singlestranded pieces. Similar, single-stranded fragments are also made
from labelled DNA of strain A. Under appropriate conditions,
the unlabelled, single-stranded DNA from strain A (which
is bound to the membrane) is then exposed to the singlestranded fragments from strains A and B; the concentration of
B fragments is very much higher than that of the A fragments.
This allows the fragments to hybridize, by base-pairing, with
complementary sequences in the bound DNA.
The fragments from strains A and B compete for sequences
on the bound DNA. However, the concentration of B fragments
is very much higher than that of A fragments; consequently, if
strains A and B are very similar, few (if any) of the (labelled )
A fragments will hybridize. On the other hand, if strains A and
B are very different many of the A fragments will hybridize.
Thus, the similarity between strains A and B is indicated by the
number of A fragments which hybridize; this can be determined
by measuring the label on the A fragments after all unbound
fragments have been washed away. Such an assay requires
controls; in one control, the assay is carried out with only
labelled A fragments this indicating the maximum amount of
binding by A fragments. Results are meaningful only if the
A fragments hybridize stably; the stability of binding can be
assessed by monitoring the dissociation of A fragments from
the bound DNA as the temperature is gradually raised.
Homology may also be assessed by comparing the thermal
stability of HETERODUPLEXes formed from two samples of DNA
DNA polymerase
this capacity and requires longer incubation times compared with
a reverse transcriptase [EMBO (1993) 12 387396].
Polymerase II (polB product) is induced in the SOS SYSTEM
(q.v.).
Polymerase III is the main replicative enzyme in E. coli
and is responsible for replication of the chromosome and of
phage DNA etc. DNA polymerase III refers to a core enzyme
consisting of three different subunits: (i) subunit a (product of
dnaE /polC ), which is involved in polymerization; (ii) subunit e
(product of dnaQ/mutD), which has 3 -to-5 exonuclease activity
and is apparently involved in proof-reading [PNAS (1983) 80
70857089] (see also MUTATOR GENE); and (iii) q (of unknown
function).
The core enzyme of polymerase III can catalyse limited DNA
synthesis on single-stranded gaps in dsDNA, but for full efficiency, accuracy and processivity on longer templates it requires
a number of additional subunits which include: (i) the b subunit (dnaN product; ?Factor I), which apparently contributes
to processivity; (ii) the g subunit (dnaZ product), which apparently also contributes to processivity; (iii) the d subunit (dnaX
product; ?Factor III), which apparently enhances processivity;
and (iv) the t subunit (product of the dnaX-Z region), which acts
as a link between two core enzymes. The core enzyme together
with the full range of subunits is called DNA polymerase III
holoenzyme. (DNA polymerase III refers to the holoenzyme
minus the b subunit. DNA polymerase III refers to a complex
of core enzyme plus the t subunit.)
In a current model of DNA replication, the holoenzyme
functions as a dimer the enzymes being physically linked
via their t subunits; during replication, one enzyme forms the
leading strand while the other forms the lagging strand, i.e. they
work in opposite directions.
In other bacteria, DNA polymerases appear to be essentially
similar to those in E. coli. In the Archaea, DNA polymerases
may be significantly different (see e.g. APHIDICOLIN).
In some prokaryotes (those that inhabit high-temperature
environments), the DNA polymerases are thermostable, and
this feature is exploited in various techniques used for the
amplification of nucleic acids in vitro (e.g. PCR); these enzymes
include:
(a) Taq DNA polymerase. An enzyme (from the bacterium
Thermus aquaticus) which has been widely used in PCR
(particularly during the early years); this enzyme lacks 3 -to5 exonuclease activity and (therefore) has no proof-reading
capacity.
(b) Stoffel fragment. A modified, recombinant form of the
Taq polymerase (the C-terminal region of the protein) which is
more thermostable than the parent enzyme; it lacks 5 -to-3 (in
addition to 3 -to-5 ) exonuclease activity. This enzyme is active
in a wide range of concentrations of magnesium ions, and has
been found useful e.g. in those forms of PCR which use arbitrary
primers.
(c) UlTma DNA polymerase (Perkin-Elmer). This recombinant form of the DNA polymerase of Thermotoga maritima has
3 -to-5 exonuclease activity and can repair 3 mismatches during PCR such proof-reading ability making the enzyme useful
for high-fidelity copying.
(d) Pfu DNA polymerase (Stratagene). This highly thermostable enzyme from Pyrococcus furiosus retains 95% activity
after 1 hour at 98 C; it has excellent proof-reading ability.
Eukaryotic DNA polymerases. Eukaryotes also have a number
of DNA polymerases, including (in most eukaryotic cells)
polymerases a, b and g. Each type of polymerase appears to
DNA polymerase I
be associated with a particular function for example, the g
polymerase carries out DNA replication in mitochondria.
Some viruses (e.g. bacteriophage T4) encode their own DNA
polymerases; others (e.g. phages fd, fX174, G4) use host
enzymes.
DNA polymerase I (Kornberg enzyme) In Escherichia coli : an
enzyme associated e.g. with EXCISION REPAIR and with the
removal of RNA primers during DNA replication. (See also DNA
POLYMERASE.)
DNA polymerase II In Escherichia coli : a polymerase induced
in the SOS SYSTEM. (See also DNA POLYMERASE.)
DNA polymerase III In Escherichia coli : the major DNA polymerase; it is involved in chromosomal replication and e.g.
synthesis of phage DNA. For further details see entry DNA POLYMERASE.
DNA polymerase IV In Escherichia coli : the product of gene
dinB (induced in the SOS SYSTEM), a protein which has DNA
polymerase activity and which appears to be involved in
mutagenesis; DinB has no proof-reading activity.
DNA polymerase V In Escherichia coli : a protein complex,
consisting of two UmuD proteins and one UmuC protein, which
has DNA polymerase activity and which may carry out some
instances of DNA repair (translesion synthesis) during induction
of the SOS SYSTEM.
DNA polymorphism See POLYMORPHISM (sense 3).
DNA primase Syn. PRIMASE.
DNA repair Any physiological process in which damaged DNA
within a cell is recognized and repaired; damage in this
context generally means any alteration or distortion of the
normal double-helical structure of dsDNA resulting e.g. from
the presence of abnormal bases or base pairs, nicks or gaps in
one strand, covalent linkages between bases etc. (but not from
replacement of one normal base pair with another: cf. MUTATION).
Repair may involve e.g. direct reversal of the damage (e.g. Ada
protein in ADAPTIVE RESPONSE) or removal of the damaged region
followed by its replacement with normal DNA (e.g. EXCISION
REPAIR).
Repair systems may be constitutive or inducible.
See e.g. ADAPTIVE RESPONSE, BASE EXCISION REPAIR, EXCISION
REPAIR, MISMATCH REPAIR, PHOTOREACTIVATION, RECOMBINATION
REPAIR and SOS SYSTEM.
DNA replication The process in which a copy (i.e. a replica) of
a double-stranded DNA molecule is synthesized.
In vivo, circular, dsDNA molecules may be replicated by
the CAIRNS MECHANISMS or the ROLLING CIRCLE MECHANISM; the
following refers mainly to the replication of circular dsDNA
molecules by the Cairns mechanism (replication of linear
dsDNA is also considered briefly). (For replication of DNA in
vitro see e.g. PCR and SDA.)
During replication, a new strand of DNA is synthesized on
each of the two pre-existing strands, each pre-existing strand
being used as a pattern or template; a template dictates the
sequence of nucleotides in a new strand, thus conserving the
genetic information encoded in the template strand. Essentially,
molecules of deoxyribonucleoside triphosphate (dNTPs) basepair with complementary nucleotides in each template strand
and are sequentially polymerized (with elimination of pyrophosphate) by a DNA POLYMERASE. Note that each newly synthesized
strand is complementary to not a copy of the template strand
on which it is synthesized; thus, each of the two new daughter
duplexes produced from a given parent duplex consists of one
parent strand and one newly synthesized strand. (This type of
replication is called semiconservative replication because only
one strand in each daughter duplex has been newly synthesized.)
DNA replication
3
5
primer
'leading' strand
DNA duplex
5
3
2nd primer
Okazaki
fragment
1st primer
3
5
3
5
DNA REPLICATION (Cairns-type): disposition of template and newly synthesized strands at a replication fork (diagrammatic; see entry). In a
circular DNA duplex the strands have separated, locally, in the ori region. Only one half of this region is shown; in this half, the strands of
the duplex will continue to separate in a left right direction (i.e. the replication fork is moving to the right). On one template strand (top) an
RNA primer (zigzag line) has been synthesized (see text); ongoing addition of deoxyribonucleotides to the 3 end of this primer will form the
leading strand of DNA. Synthesis of the leading strand is continuous in the 5 -to-3 direction.
On the other template strand (below), the 1st primer has been synthesized (by a primase), and this (RNA) primer has been extended as a
strand of DNA by sequential addition of deoxyribonucleotides from the 3 end. This new strand of DNA may form the first Okazaki fragment
of the lagging strand; alternatively, it may act as a primer for leading strand synthesis in the other replication fork (not shown). Following
synthesis of the 1st primer, the replication fork has moved further to the right opening up the duplex to the extent shown in the diagram. The
2nd primer has been synthesized and has been extended as a strand of DNA (Okazaki fragment) as far as the 5 end of the first primer. As the
replication fork moves even further to the right additional template will become available, and the 3rd, 4th, 5th . . . etc. primers synthesized on
this template will (like the 2nd primer) be extended as Okazaki fragments; the sequence of Okazaki fragments will be joined together (forming
the lagging strand) when the (RNA) primers are replaced by DNA.
Modified from Bacteria, 5th edition, Figure 7.8(a), page 116, Paul Singleton (1999) copyright John Wiley & Sons Ltd, Chichester, UK (ISBN
0471-98880-4) with permission from the publisher.
DNA restriction
most or all cases at least some of the components involved in
host chromosomal replication are required.
In plasmid ColE1, replication is of the Cairns type but
it occurs unidirectionally from the origin; in the F PLASMID
replication is bidirectional (as in the E. coli chromosome).
Many of the small circular plasmids in Gram-positive bacteria
replicate by means of a ROLLING CIRCLE MECHANISM [replication
control in rolling circle plasmids: TIM (1997) 5 440446].
Plasmid replication, and the partitioning to daughter cells,
seems likely to involve some kind of association between the
plasmid and the cytoplasmic membrane of the host cell [Mol.
Microbiol. (1997) 23 110].
Replication of the (linear) genome of bacteriophage f29 was
mentioned above.
In certain phages the rolling circle mechanism is involved in
replication (see e.g. SSDNA PHAGE, BACTERIOPHAGE l, BACTERIOPHAGE fX174).
[The enzymology of DNA replication (historical perspective):
JB (2000) 182 36133618.]
DNA restriction See RESTRICTIONMODIFICATION SYSTEM.
DNA sequencing Any procedure for determining the sequence
of nucleotides in a sample of DNA. Sequencing is important in
taxonomy, identification and characterization.
In the chemical (MaxamGilbert) method, end-labelled
copies of an unknown sequence are cleaved by base-specific
reagents; analysis follows electrophoresis of the fragments. The
dideoxy (Sangers) method is described in the figure on page
249. (See also PYROSEQUENCING.)
Automated DNA sequencing is often based on the dideoxy
method. Primers are labelled with fluorescent dyes, a different
dye being used for each of the four reactions. The products
from all four reactions are combined and then subjected to
electrophoresis from a single well in a polyacrylamide gel.
On excitation by an argon laser, fragments from each reaction
mixture can be distinguished from those of other reaction
mixtures by their dye-specific emission characteristics; emissions
from the fragments of all four reaction mixtures are detected
automatically and stored e.g. in digital form.
Sequencing provides definitive information on a given sample
of nucleic acid. For duplex DNA, greater accuracy is obtained
if both strands of the duplex are sequenced.
RNA can be retrotranscribed into cDNA; the (single-stranded)
cDNA is then amplified, and the amplified product is sequenced.
The sequence of nucleotides in the RNA sample is then deduced.
Amplified DNA copies of an RNA sample may be obtained by
reverse-transcriptase PCR (rtPCR).
DNA splicing See CLONING (of DNA).
DNA Stat See BLOOD DNA ISOLATION KITS.
DNA synthesis See DNA REPLICATION.
DNA topoisomerase Syn. TOPOISOMERASE.
DNA toroid A highly compacted genomic DNA, found e.g. in
Deinococcus radiodurans and ENDOSPORES, which may account
at least partly for resistance to DNA-damaging agents (e.g.
radiation). Toroidal structure may facilitate repair of doublestranded breaks in a RecA- and template-independent way [JB
(2004) 186 59735977].
DNA tumour viruses Oncogenic DNA-containing animal viruses; they include members of the ADENOVIRIDAE, Hepadnaviridae (see e.g. HEPATITIS B VIRUS), Herpesviridae (subfamily GAMMAHERPESVIRINAE), and PAPOVAVIRIDAE.
DNA unwinding protein Any protein capable of unwinding and
separating the strands of double-helical DNA. (See HELICASES;
cf. SINGLE-STRAND BINDING PROTEIN.)
TCTGACGTAAGC
ddG
ddC
ddT
ddA
T
C
T
G
A
C
G
T
A
A
G
C
DNA SEQUENCING: determining the nucleotide sequence of a cloned DNA fragment by the dideoxy method (Sangers chain-termination
method) (diagrammatic). Initially, the fragment to be sequenced is obtained in single-stranded form (e.g. by cloning in a phage M13 vector).
Regardless of the cloning method used, the unknown sequence will be flanked on its 3 side by single-stranded DNA of known sequence
derived from the vector molecule; this permits the design of a labelled primer which can bind at a site next to the unknown sequence such
that the first nucleotide to be added to the primer will pair with the first 3 nucleotide of the unknown sequence. In the diagram, the unknown
sequence is TCTGACGTAAGC; a primer (short line), which carries a label (black disc), has bound at a site flanking the 3 end of the unknown
sequence.
DNA synthesis in vitro is normally carried out with a reaction mixture that includes (i) templates (in this case, single-stranded fragments
containing the unknown sequence); (ii) primers; (iii) the four types of deoxyribonucleoside triphosphate (dATP, dCTP, dGTP and dTTP); and
(iv) DNA polymerase. When base-paired to the template strand, the primer is extended (5 -to-3 ) by the sequential addition of nucleotides as
dictated by the template.
In sequencing, there are four separate reaction mixtures (G, C, T, A), each containing all the constituents mentioned above (including
millions of copies of the unknown sequence, and of the primer). In addition, each mixture contains a given dideoxyribonucleoside triphosphate
(ddNTP); thus, the G mixture contains dideoxyguanosine triphosphate (ddG), the C mixture ddC, the T mixture ddT, and the A mixture ddA.
When a dideoxyribonucleotide is added to a growing strand of DNA it prevents addition of the subsequent nucleotide because
dideoxyribonucleotides lack the 3 -OH group necessary for making the next phosphodiester bond. Thus, primer extension will stop (=
chain termination) at any location where a dideoxyribonucleotide has been incorporated. In each reaction mixture the concentration of ddNTP
is such that, in most growing strands, synthesis will be stopped, at some stage, by the incorporation of a dideoxyribonucleotide; because a
ddNTP may pair with any complementary base in the template, chain termination can occur at different sites on different copies of the template
strand so that product strands of different lengths will be formed. For example, with ddG (see diagram) the three products are of different
lengths because, during extension of the primers, ddG has paired with cytosine residues at three different locations in the template; note that,
in this case, the length of a given product strand is related to the location of a particular cytosine residue in the unknown sequence. Analogous
comments apply to reaction mixtures containing the other ddNTPs.
At the end of the reaction, product strands are separated from templates by formamide. Each reaction mixture is then subjected to
electrophoresis in a separate lane of a polyacrylamide gel. Short product strands move further than longer ones, in a given time; products that
differ in length by only one nucleotide can be distinguished, the shorter product moving just a little further.
The gel contains urea; this inhibits base-pairing between product strands and templates. It also inhibits intra-strand base-pairing in the
product strands. This is essential: to deduce the sites of a particular base in the template it is necessary to compare the lengths of all
product strands in the given reaction, and this requires proportionality between strand length and electrophoretic mobility; were intra-strand
base-pairing to occur it could alter electrophoretic mobility in which case a products length would not necessarily be indicated by the
position of its band in the gel. (Continued on page 250.)
249
250
dot-blot
Domestos See HYPOCHLORITES.
dominance (genetics) In a diploid (or merodiploid) heterozygous
cell or organism: the tendency of certain (dominant) alleles to
be expressed in preference to their corresponding (recessive)
alleles. (cf. EPISTASIS.) The complete dominance of one allele
over another occurs in only some cases; in such cases the
phenotype of the heterozygote Aa is identical to that of the
homozygote, AA (A being dominant). When partial dominance
is exhibited the Aa phenotype is intermediate between the AA
and aa phenotypes.
dominant allele See DOMINANCE.
Domiphen bromide See QUATERNARY AMMONIUM COMPOUNDS.
DON (1) (6-diazo-5-oxo-L-norleucine; CO2 H.CHNH2 .(CH2 )2 .
CO.CH=N+ =N ) An ANTIBIOTIC and antitumour agent obtained
from Streptomyces sp; its mode of action resembles that of
AZASERINE. Other antitumour DON derivatives are produced
by Streptomyces spp: e.g. diazomycin A (N-acetyl-DON) and
alazopeptin (apparently comprising one alanine and two DON
residues). (cf. HADACIDIN.)
(2) Deoxynivalenol see TRICHOTHECENES.
donation (mol. biol.) See CONJUGATION (1b) (i).
donor Any cell or organism which donates genetic information
to another cell or organism (the recipient): see CONJUGATION,
TRANSDUCTION and TRANSFORMATION.
donor conjugal DNA synthesis See CONJUGATION (1b) (i).
donor site (of a ribosome) See PROTEIN SYNTHESIS.
donor splice site See SPLIT GENE (a).
donor-suicide model (for transposition) See e.g. Tn10.
Donovan bodies See GRANULOMA INGUINALE.
donovanosis Syn. GRANULOMA INGUINALE.
L-dopa See MELANIN.
Dorisa See EIMERIORINA.
Dorisella See EIMERIORINA.
dormancy (hypobiosis) The state of an organism or spore which
exhibits minimal physical and chemical change over an extended
period of time; when no physical or chemical change can be
detected the state is sometimes referred to as cryptobiosis. (See
also ENDOSPORE (sense 1(a)) and SPORE.)
dorsal zone of membranelles See DZM.
Dorsets egg A MEDIUM used e.g. for the maintenance of Mycobacterium spp; it consists of a saline suspension of homogenized
whole hens eggs which has been inspissated in sloped bijou or
universal bottles.
dorsiventral Having two unlike (upper and lower) surfaces.
dosa A traditional fermented food in India; it is prepared from
milled rice and black gram (cf. IDLI). [Microbiology of dosa:
Food Mic. (1986) 3 4553.]
dosage (of genes) See GENE DOSAGE.
dot-blot A PROBE-based method for detecting or quantifying a
specific sequence of nucleotides in a given sample. A drop of
the sample is added to a suitable membrane and treated so that
any nucleic acids present in the sample bind to the membrane in
single-stranded form. The membrane is then exposed to probes
(which are complementary to the target sequence) under conditions permitting probetarget hybridization; when unbound
probes are removed by washing, the presence of bound probes
indicates the presence of the required target sequence. If, for
example, the probe had been tagged with DIGOXIGENIN, the bound
probe is detected by treating the membrane with a conjugate consisting of anti-digoxigenin (antibody to digoxigenin) covalently
linked to an enzyme (such as alkaline phosphatase); the binding
of conjugate to digoxigenin is determined by adding a colourgenerating substrate for the enzyme after all unbound conjugate
has been removed by washing.
dot genes
downstream box In certain prokaryotic and phage genes: a
sequence of nucleotides, downstream from the start site, which
has been regarded as a translation enhancer. The ribosomal
16S rRNA may contain a complementary region (called the
anti-downstream box ), although suggestions that this may bind
to the downstream box have been disputed [JB (2001) 183
34993505].
downstream promoter element In some RNA polymerase II
PROMOTERS: a region downstream of the start site with a role
apparently similar to that of the TATA box.
downy mildews Plant diseases caused by certain members of
the PERONOSPORALES (e.g. BREMIA, PERONOSPORA, PLASMOPARA);
downy mildews are characterized by the formation of superficial
hyphal growth in which, typically, individual spore-bearing
structures can be distinguished under low magnification. (cf.
POWDERY MILDEWS.) Downy mildews can be controlled e.g. with
copper-based antifungals or ZINEB.
doxycycline See TETRACYCLINES.
Dp Pattern difference. In the comparison of two strains by
NUMERICAL TAXONOMY: a coefficient which indicates the degree
of dissimilarity corrected for any difference(s) due solely to
inter-strain differences in metabolic vigour. (cf. entry Sp .)
DP Degree of polymerization: the number of monomeric units
per molecule of a polymer.
DPD N,N-diethyl-p-phenylenediamine (see WATER SUPPLIES).
DPN Diphosphopyridine nucleotide: see NAD.
DPT A MIXED VACCINE containing diphtheria toxoid, pertussis
vaccine and tetanus toxoid.
DPX A neutral, synthetic MOUNTANT of refractive index ca. 1.53
when dry; it consists of Distrene and a plasticizer (tritolyl
phosphate) dissolved in x ylol.
DR DIRECT REPEAT.
Dr adhesins A category that includes both fimbrial and nonfimbrial adhesins, members of which are found e.g. on UPEC
strains of Escherichia coli; the Dr adhesins bind to CD55 (at a
site corresponding to the Dra blood group antigen).
draft tube In a LOOP FERMENTER: a wide, vertical tube typically
situated coaxially within the column so as to leave an annular
space between itself and the wall of the fermenter; when the
fermenter is operating, the draft tube is completely submerged
in the culture. Culture is made to flow up (or down) the draft tube
in order to generate a circulatory flow in the column culture
flowing down (or up) the annulus.
DraI See RESTRICTION ENDONUCLEASE (table).
Draparnaldia See CHAETOPHORA.
draughtsman colony (checker colony) The form of COLONY
typically (though not invariably) produced by Streptococcus
pneumoniae growing on blood agar: round and raised, with steep
sides and a flat top, i.e., resembling one of the pieces used in a
game of draughts (= checkers); after overnight growth under a
raised partial pressure of CO2 the colonies are each ca. 1 mm
in diameter and surrounded by a zone of a-haemolysis. Very
young colonies of S. pneumoniae are typically convex (domed);
the flattened colony form apparently results from autolysis of the
constituent cells on continued incubation, and further incubation
may result in the development of a concavity in the upper surface
of the colony.
draw tube In some microscopes: a tube coaxial with the body
tube (see MICROSCOPY) used to adjust the tube length.
drd plasmid
A mutant CONJUGATIVE PLASMID in which the
TRANSFER OPERON is permanently DEREPRESSED.
Drechslera
A genus of fungi of the HYPHOMYCETES; teleomorphs occur in the genera Cochliobolus and Pyrenophora.
Dunaliella
The organisms form septate mycelium and pigmented, septate, commonly cylindrical conidia; conidiogenesis is tretic (see
CONIDIUM). Drechslera spp are typically graminicolous (cf. e.g.
PHAEOHYPHOMYCOSIS). Species which have been transferred from
HELMINTHOSPORIUM to this genus include e.g. D. gramineae,
D. maydis, D. oryzae (causal agent of brown spot disease of
rice), and D. victoriae (see also VICTORIN).
Dreyers tube A small, conically-based glass test-tube with a
flared rim and an internal diameter of ca. 5 mm; it is used
in serology for the clear observation of reactions involving
agglutination or precipitation.
drift See GENETIC DRIFT and ANTIGENIC DRIFT.
DRNA DISSIMILATORY REDUCTION OF NITRATE TO AMMONIA.
drop plate method Syn. MILES AND MISRAS METHOD.
droplet infection INFECTION (sense 1) by inhalation of an AEROSOL of saliva, mucus etc. (contaminated with pathogens) from
an infected individual.
dropsy Syn. OEDEMA. (See also INFECTIOUS DROPSY.)
Drosophila A virus See PICORNAVIRIDAE.
Drosophila C virus See PICORNAVIRIDAE.
Drosophila P virus See PICORNAVIRIDAE.
Drosophila X virus (DXV) A virus which causes anoxia sensitivity and death in Drosophila melanogaster and which can be
cultivated in Drosophila cell lines [JGV (1979) 42 241254].
DXV closely resembles IPN VIRUS in morphology, genome etc.
(See also SIGMA VIRUS.)
drug resistance Syn. ANTIBIOTIC resistance.
dry bubble See BUBBLE DISEASES.
dry rot (1) (of timber) A BROWN ROT of structural (and other)
timbers caused by the cellulolytic fungus Serpula lacrymans;
only wood having a moisture content greater than about 20% (see
TIMBER SPOILAGE) can be attacked initially, but water produced
during metabolism can be transported via moisture-conducting
rhizomorphs, enabling the fungus to spread to drier regions of
wood (or across brickwork etc). Infected timbers often exhibit
longitudinal and cross-grain cracking and a surface growth of
whitish mycelium containing yellow and/or lilac patches; the
leathery fruiting bodies bear a mass of rust-coloured spores.
Control of dry rot involves removal of decayed wood and
disinfection of remaining timbers by heat and/or the application
of fungicides (see TIMBER PRESERVATION). Infections similar to
dry rot may be caused e.g. by Poria spp. (cf. WET ROT.)
(2) A storage rot of potato tubers caused e.g. by Fusarium
coeruleum ( = F. solani var. coeruleum) and F. sulphureum.
The tubers develop dark, sunken lesions which develop into
mycelium-filled cavities; affected tubers lose water and shrink,
becoming wrinkled and eventually drying into a hard mass.
Under humid conditions, however, infection by SOFT ROT organisms may result in rapid decomposition of the tubers. (See also
TECNAZENE.)
dryads saddle Polyporus squamosus (q.v.).
drying (1) (of foods) See FOOD PRESERVATION (c). (2) (of plates)
See PLATE. (3) (of microorganisms) See DESICCATION.
ds (of DNA or RNA) Double-stranded.
dsb genes See PROTEIN SYNTHESIS (protein folding).
ds(c)DNA Double-stranded circular DNA.
DSI stain See DIETERLE SILVER STAIN.
DSM Deutsche Sammlung von Mikroorganismen (culture collection of microorganisms), Grisebachstr. 8, D-3400 Gottingen,
Germany.
DTH Delayed-type hypersensitivity: see DELAYED HYPERSENSITIVITY.
dTMP Deoxythymidine 5 -monophosphate [see Appendix V(b)].
Duncan disease
10 distinct dsRNA segments whereas healthy isolates contain
04 dsRNA segments, suggesting that specific dsRNA segments
may be associated with the development of disease [PP (1986)
35 277287]. (See also CHESTNUT BLIGHT and MYCOVIRUS.)
Duttonella A subgenus of TRYPANOSOMA within the SALIVARIA;
species include parasites and pathogens of a range of wild and
domestic animals (see e.g. NAGANA). The trypomastigote form
typically has a large, terminal kinetoplast and a free flagellum.
T. (D.) vivax occurs in the vertebrate in the trypomastigote
form (ca. 2030 m in length) which divides by longitudinal
binary fission; it is transmitted cyclically by Glossina spp in
which epimastigotes and metacyclic forms develop solely in the
proboscis. Mechanical transmission by other biting flies (e.g.
Tabanus) occurs outside the tsetse belt.
T. (D.) uniforme is similar to T. (D.) vivax, though somewhat
smaller.
Duvals bacillus Shigella sonnei.
Duvenhage virus See LYSSAVIRUS.
DVH DUCK VIRUS HEPATITIS.
dw Dry weight.
dwarf bunt See COMMON BUNT.
DWELL See ETRIDIAZOLE.
dyad symmetry See e.g. PALINDROMIC SEQUENCE.
dye A water-soluble, aromatic compound which has coloured
anions and/or cations that can bind to particular substance(s);
binding may be primarily ionic but may involve e.g. hydrogenbonding. (See also AUXOCHROME; CHROMOPHORE; LEUCO COMPOUND.) (In microbiology dye is often used interchangeably
with stain to refer not only to dyes, as defined, but also to other
substances e.g. LYSOCHROMES used for STAINING; stain may
also refer to a mixture of dyes and/or to the process of using a
dye or stain.) An acid dye has a coloured anion which combines
with cationic groups. A basic dye has a coloured cation which
combines with anionic groups. A neutral dye is a compound of
acid and basic dyes in which each ion contains a chromophore.
(The pH of a solution of such dyes does not necessarily indicate whether the dye is acid, basic or neutral.) An amphoteric
dye is either acidic or basic according to pH. Although dyes are
commonly used for STAINING, some have additional uses: see
e.g. ACRIDINES, ETHIDIUM BROMIDE, METHYLENE BLUE, TRIPHENYLMETHANE DYES; see also PH INDICATORS, RESAZURIN TEST.
Dyes are classified according to the nature of their chromophores. Those based on a (para- or ortho-) quinonoid ring
include the TRIPHENYLMETHANE DYES, xanthene dyes (e.g. EOSIN,
pyronin), azine dyes (e.g. JANUS GREEN, NEUTRAL RED, NIGROSIN),
azine-related dyes (oxazines, e.g. NILE BLUE A; thiazines, e.g.
METHYLENE BLUE, thionin, toluidine blue), and HAEMATEIN. Dyes
with a chromophore of one or more azo groups (N=N) include
BISMARCK BROWN, CHLORAZOL BLACK E, CONGO RED and TRYPAN
BLUE; Janus green also contains an azo group. Dyes with a nitro
group as chromophore include 2,4,6-trinitrophenol (picric acid).
dye-buoyant density centrifugation See ultracentrifugation in
the entry CENTRIFUGATION.
dye test Syn. TOXOPLASMA DYE TEST.
Dynabeads Microscopic beads used in magnetic separation:
a technique in which a particular type of cell or molecule is
separated from a mixture (in the liquid phase) by allowing the
required cells or molecules to bind to beads coated with a specific
ligand the beads then being segregated by use of a magnetic
field.
Dynabeads (Dynal, Skyen, Oslo, Norway) are microscopic
spheres that contain a mixture of iron oxides; they are superparamagnetic, i.e. they do not exhibit magnetic properties until
dysentery
placed in a magnetic field. The beads can be coated with any of
a variety of ligands the particular type used depending on the
required cell or molecule. For example, if beads are coated with
the oligonucleotide T-T-T-T-T-T-T they will bind the poly-A
tails of mRNA molecules; this approach can be used to separate
mRNAs from total RNA.
Essentially, the beads are well dispersed within the sample
by thorough mixing; the required cells or molecules bind to
the beads which are then drawn to one side of the vessel
by a magnetic field. Unwanted material is discarded, and the
required cells/molecules can be washed etc. prior to use. (Note
that permanently magnetic beads would not be suitable: they
would clump together rather than disperse within the sample.)
Beads coated with specific antibodies are useful for isolating particular pathogens E. coli O157, Salmonella spp, Listeria monocytogenes etc. from food or other specimens; the
beadpathogen complex can be plated on a suitable medium.
This approach can also be used to isolate a specific type of
eukaryotic cell from a mixture of cells. This method is called
immunomagnetic separation (IMS).
Examples of use include: enrichment of Mycobacterium
paratuberculosis in milk [AEM (1998) 64 31533158]; detection of E. coli O157 in meat [LAM (1998) 26 199204];
preparation of human glomerular endothelial cells for use in
tests with E. coli verocytotoxin [Kidney International (1997) 51
12451256]; detection of specific mycobacterial DNA prior to
PCR (sequence capture PCR) [JCM (1996) 34 12091256].
dynein See FLAGELLUM (b).
dysentery A disease characterized by inflammation of the intestine (particularly the colon), abdominal pain, and frequent passage of fluid stools that may contain blood, mucus and/or pus.
Dysentery (rather than DIARRHOEA) is the term generally used
to refer to a diarrhoeal condition in which (i) blood/mucus is
typically present in the stool, and (ii) the intestinal epithelium
is actively invaded by the causative organism (as is the case with
e.g. Shigella dysenteriae, enteroinvasive E. coli and Entamoeba
histolytica).
(1) (med.) (a) Bacillary dysentery. The classical (severe) form
of dysentery is caused by Shigella dysenteriae serotype 1 (found
mainly in tropical countries); somewhat less severe disease
is caused by S. sonnei (a common causal agent in temperate
zones), S. boydii (mostly tropical) and S. flexneri. As well as
the shigellosis, caused by Shigella spp, bacillary dysentery can
be caused e.g. by EIEC.
Dysentery caused by S. dysenteriae type 1 is transmitted via
the faecaloral route commonly via food or water contaminated with faeces from patients with dysentery (or from a
carrier of the pathogen). Incubation period: 16 days. Onset is
abrupt, with fever followed by diarrhoea and abdominal cramps.
S. dysenteriae proliferates in the gut lumen and invades the
epithelium of the terminal ileum and colon. While dysentery
due to S. sonnei and S. boydii is typically self-limiting (lasting
days), that caused by S. dysenteriae may cause ulceration of the
intestinal mucosa and may last for weeks, leading to exhaustion
and anaemia; mortality may be high in untreated cases.
In animal studies, Shigella is taken up via the so-called
M cells in Peyers patches [M cells in infection (review):
TIM (1998) 6 359365]; from this location the bacteria can
spread from cell to cell within the epithelial layer. Such
spreading (an essential feature of dysentery) depends on the
presence of a (plasmid-encoded) outer membrane protein: IcsA
(= VirG). (IcsA is the a-domain of an autotransporter: see
type IV secretory systems in PROTEIN SECRETION. An analogous
dysgonic
(2) (vet.) See e.g. LAMB DYSENTERY, SWINE DYSENTERY, WINTER
(cf. SCOURS.)
dysgonic See EUGONIC.
dyskinetoplasty In e.g. certain naturally-occurring strains of
Trypanosoma evansi : the absence of a normal KINETOPLAST the
mitochondrion containing, instead, a small, spherical, electrondense body, the kinetoplast remnant, which is not visible
in Giemsa-stained preparations. Dyskinetoplastic strains of T.
evansi and other trypanosomes can be obtained by exposure to
e.g. Berenil.
dysphotic zone See PHOTIC ZONE.
dyspnoea (dyspnea) Difficult or laboured breathing.
Dysteria See HYPOSTOMATIA.
DZM Dorsal zone of membranelles: a SYNCILIUM (or syncilia)
occurring in the anteriodorsal region of some ciliates, e.g.
Diplodinium, Epidinium.
DYSENTERY.
256
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
E
Corynebacterium, Mycobacterium and various yeasts. (See also
BODY MICROFLORA.)
Earles BSS Earles BALANCED SALT SOLUTION; it contains (g/l):
NaCl (6.8), KCl (0.4), MgSO4 .7H2 O (0.2), NaH2 PO4 .2H2 O
(0.158), CaCl2 .2H2 O (0.264), NaHCO3 (2.2), glucose (1.0), and
phenol red (0.01); pH: 7.67.8.
early blight (of potato) A POTATO DISEASE caused by Alternaria
solani. Small dark spots appear on leaves, each spot having
concentric rings of necrotic tissue which give a characteristic
target appearance; tubers may exhibit a superficial brown, dry,
corky rot.
early genes See VIRUS.
earth balls See SCLERODERMATALES.
earth stars See LYCOPERDALES.
earth tongues Fruiting bodies of species of e.g. Geoglossum or
Trichoglossum.
East Coast fever An East African tick-borne disease of cattle
caused by species of THEILERIA; T. parva and T. lawrencei
cause a febrile disease which is usually fatal, while T. mutans
typically causes non-febrile anaemia which may be fatal. After
the tick vector has ingested blood from an infected bovine
host, sexual stages of Theileria appear in the ticks gut;
zygotes develop in the gut, and each forms a motile kinete
which migrates to the ticks salivary glands and undergoes
schizogony to form infective sporozoites. The tick can then
infect a fresh bovine host. In the new (vertebrate) host the
parasite grows in fixed and/or circulating lymphoid cells and
forms macroschizonts (Kochs blue bodies; blue bodies):
schizonts, 1020 m in size, whose cytoplasm stains blue
with Giemsas stain. Subsequently, intra-erythrocytic forms
(piroplasms) of T. parva (or T. mutans) become common, but
may be scanty/undetectable in T. lawrencei. T. parva and T.
lawrencei infections usually kill after 15 days. [Life cycles of
Babesia and Theileria: AP (1984) 23 37103. Anti-T. parva
vaccine: Annals New York Acad Sci (2000) 916 464473.]
EAST 1 A heat-stable toxin secreted e.g. by EAGGEC, many
strains of EHEC O157:H7, and by Yersinia enterocolitica; it is an
analogue of the endocrine hormone guanylin (which stimulates
fluid outflow from the intestinal mucosa by activating guanylyl
cyclase).
eastern equine encephalomyelitis (EEE; eastern equine encephalitis; eastern encephalitis) An acute ENCEPHALITIS (or encephalomyelitis) of man and horses, caused by an ALPHAVIRUS; it occurs
in eastern North America, the Caribbean, and parts of Central
and South America. EEE virus can also cause disease in domestic birds (pigeons, pheasants). The virus occurs in wild birds, in
which transmission occurs mainly via Culiseta melanura; other
mosquitoes (e.g. Aedes spp) may be responsible for the sporadic
transmission of EEE to animals and man. In man, the mortality
rate may be ca. 2570% or higher. Epizootics in horses may be
controlled by vaccination.
Eatons agent Mycoplasma pneumoniae.
EB ELEMENTARY BODY.
EB virus EPSTEINBARR VIRUS.
EBERs (EBV) See EPSTEINBARR VIRUS.
ebna genes (EBV) See EPSTEINBARR VIRUS.
Ebola virus See FILOVIRIDAE.
EBV EPSTEINBARR VIRUS.
E (1) See REDOX POTENTIAL. (2) Glutamic acid (see AMINO ACIDS).
E-cadherin See CADHERINS.
E. coli An abbreviation which usually refers to the bacterium
Escherichia coli (see entry ESCHERICHIA) but which is also used
e.g. for the protozoan Entamoeba coli. (This illustrates the need
to ensure that the name of a genus is spelt out in full on first
usage before using an abbreviated form.)
E precursor cells (immunol.) Cells on whose surface COMPLEMENT FIXATION has occurred, at 4 C, but which do not lyse unless
the temperature is raised; lysis can be further inhibited, even at
higher temperatures, by EDTA or zinc or uranyl salts.
E protein See F PLASMID.
E-selectin Syn. CD62E.
E site (of a ribosome) See PROTEIN SYNTHESIS.
E test A diffusion test for determining the MIC of a given
bacterial strain with respect to particular antibiotic(s). One side
of a plastic strip (placed in contact with the inoculated plate)
carries a given antibiotic, the concentration of which decreases
uniformly from one end of the strip; the other side of the
strip is graduated with the concentration of antibiotic. Following
incubation, the MIC is read by noting the lowest concentration
of antibiotic (on the scale) which corresponds to inhibition of
growth. Several strips, each with a different antibiotic, can be
used simultaneously on a standard-sized plate.
The E test has been used for various bacteria, including
Pseudomonas aeruginosa [JCM (1991) 29 533538] and [Helicobacter pylori [JCM (1997) 35 18421846]. [Mycobacterium
tuberculosis: JCM (2002) 40 22822284.]
E0 (E0 ) See REDOX POTENTIAL.
E0 See REDOX POTENTIAL.
(E1 E2 )-type H+ -ATPase See PROTON ATPASE.
e14 element See RECOMBINATIONAL REGULATION.
E5531 See ENDOTOXIC SHOCK.
EA Erythrocyteantibody (see e.g. HAEMOLYTIC SYSTEM). (cf.
EAC.)
EAC Erythrocyteantibodycomplement. EAC 142 . . . indicates
that COMPLEMENT components 142 . . . have been fixed. (cf. EA.)
eae gene See PATHOGENICITY ISLAND.
EAEC (1) ENTEROADHERENT E. COLI [RMM (1995) 6 196206].
(2) Enteroaggregative E. coli (see EAGGEC) [MR (1996) 60
167215 (p. 186)].
EAF plasmid See PATHOGENICITY ISLAND and BUNDLIN.
EAggEC Enteroaggregative Escherichia coli: strains of E. coli
associated with persistent diarrhoea usually (though not exclusively) in children in the developing countries. (See also
ENTEROADHERENT E. COLI.) The organisms form toxins and
adhesins, but the mechanism of pathogenesis is unknown.
EAggEC may be particularly important as pathogens for undernourished/immunosuppressed patients. [Enteroaggregative and
diffusely adherent E. coli: RMM (1995) 6 196206.]
Strains of O111:H12 in Brazil were reported to have the
properties of EAggEC [FEMS (1997) 146 123128].
(See also EAEC and EAST 1.)
Eagles medium Any of a number of growth or maintenance
media (used in TISSUE CULTURE) consisting basically of EARLES
BSS or HANKS BSS supplemented with e.g. amino acid(s), vitamin(s), antibiotic(s), serum etc.
ear microflora The microflora of the human ear (external auditory canal) commonly includes e.g. strains of Staphylococcus,
257
EC
with a salt concentration of ca. 330%, sulphide being oxidized
to elemental sulphur which is deposited extracellularly. Species
include e.g. E. abdelmalekii, E. halochloris, E. halophila and
E. vacuolata.
ectothrix infection See DERMATOPHYTES.
ectotrophic mycorrhiza See MYCORRHIZA.
ectotunica See BITUNICATE ASCUS.
Ectrogella See SAPROLEGNIALES.
ectromelia virus (mousepox virus) A virus (genus ORTHOPOXVIRUS) which infects mice, causing a disease (mousepox) in
which internal organs (mainly liver and spleen) are involved,
and characteristic lesions develop on the skin. Ectromelia virus
replicates slowly on the CAM, forming small, white, irregularly
shaped pocks.
eczema An inflammatory condition of the skin involving redness,
itching, development of papules and vesicles etc; it is usually an
allergic reaction. Eczema herpeticum and eczema vaccinatum are
severe, sometimes fatal, generalized conditions resulting from
disseminated infection with herpes simplex virus and vaccinia
virus, respectively; they occur most commonly in patients with
atopic dermatitis or certain immunodeficiency syndromes.
(See also PROBIOTIC)
ED pathway ENTNERDOUDOROFF PATHWAY.
ED50 Effective dose (50%): that dose of a given agent which,
when given or applied to each of a number of experimental test
animals or systems, affects 50% of those animals or systems
under given conditions.
Edam cheese See CHEESE-MAKING.
edaphic Of or pertaining to terrestrial habitats particularly soil,
but also e.g. leaf litter and the surfaces of living plants.
EDDA An iron chelator: ethylenediamine-di(o-hydroxyphenylacetic acid).
edeines A group of basic linear peptide antibiotics produced e.g.
by Bacillus brevis; they are effective against a broad spectrum of
organisms, including Gram-positive and Gram-negative bacteria,
fungi, and some mammalian cells. At low concentrations edeines
are bacteriostatic, selectively and reversibly inhibiting DNA
synthesis; at higher concentrations they may be bactericidal,
inhibiting the synthesis of proteins but apparently not of RNA.
Edelfaule (German) syn. NOBLE ROT.
edema Syn. OEDEMA.
edifenphos See HINOZAN.
editing (RNA) See RNA EDITING.
EDTA Ethylenediaminetetraacetic acid: (CH2 .N(CH2 COOH)2 )2 .
EDTA strongly chelates divalent metal ions (e.g. Zn2+ , Ca2+ ,
Mg2+ ); it is used e.g. as an ANTICOAGULANT (preventing clotting
by complexing plasma Ca2+ ) and as a potentiating agent in certain antibacterial preparations (see e.g. DETTOL CHELATE). EDTA
causes a non-specific increase in the permeability of Gramnegative bacteria, and under certain conditions it can inhibit
or lyse many Gram-negative species Pseudomonas aeruginosa
being particularly susceptible; the antibacterial activity of EDTA
may involve one or more of several phenomena: e.g., loss of
structural integrity of the OUTER MEMBRANE due to chelation
of membrane-stabilizing divalent cations, and potentiation of
peptidoglycan-degrading autolysins. EDTA has been used in the
preparation of SPHAEROPLASTS of Gram-negative bacteria (see
also OSMOTIC SHOCK). (The susceptibility of P. aeruginosa to
EDTA can be decreased by growth in Mg2+ -limited media owing
to changes in the outer membrane proteins [JGM (1983) 129
509517].) (cf. CDTA; EGTA; NTA.)
Edwardsiella A genus of Gram-negative bacteria of the ENTEROBACTERIACEAE (q.v.). Cells: ca. 1 23 m, motile (except
EC (1) Energy charge (See ADENYLATE ENERGY CHARGE). (2) Enzyme Commission (see ENZYME).
ECA ENTEROBACTERIAL COMMON ANTIGEN.
ecad A distinct population, within a given species, which has
adapted phenotypically to its environment. (cf. ECOTYPE.)
ecchymosis See PURPURA.
Eccrinales See TRICHOMYCETES.
ecdysis The shedding of an outer layer: e.g., the exoskeleton of
an invertebrate, or the theca in certain DINOFLAGELLATES.
Echinamoeba See AMOEBIDA.
echinocandin B See ACULEACIN A.
echinomycin See QUINOXALINE ANTIBIOTICS.
Echinosporangium See MUCORALES.
Echinosteliales See MYXOMYCETES.
Echinosteliopsidales See MYXOMYCETES.
Echinosteliopsis See MYXOMYCETES.
Echinostelium A genus of slime moulds (class MYXOMYCETES)
which form protoplasmodia and small, stalked sporangia
(<0.5 mm tall). E. lunatum is the smallest known myxomycete,
forming stalked sporangia <50 m tall and bearing only
48(14) spores. [Encystment of myxamoebae and protoplasmodia in E. minutum: Mycol. (1985) 77 253258.]
echinulate Covered with small spines.
echoviruses See ENTEROVIRUS.
eclipse complex See TRANSFORMATION (1).
eclipse period See ONE-STEP GROWTH EXPERIMENT.
EcoB A type I RESTRICTION ENDONUCLEASE.
EcoK A type I RESTRICTION ENDONUCLEASE.
econazole See AZOLE ANTIFUNGAL AGENTS.
Economos encephalitis Syn. VON ECONOMOS ENCEPHALITIS.
EcoPI A type III RESTRICTION ENDONUCLEASE.
EcoRI
A RESTRICTION ENDONUCLEASE from Escherichia coli ;
G/AATTC.
EcoRV See RESTRICTION ENDONUCLEASE (table).
ecotropic Refers to a (endogenous or exogenous) retrovirus
which can replicate only in hosts of the species in which it
originated. (cf. XENOTROPIC, AMPHOTROPIC.)
ecotype A distinct population, within a given species, which has
adapted genetically to its environment. (cf. ECAD.)
ectendomycorrhiza See MYCORRHIZA.
ectocarpene See PHEROMONE.
Ectocarpus See PHAEOPHYTA.
ectocyst See CYST (b).
ectomycorrhiza See MYCORRHIZA.
ectoparasite See PARASITE.
ectoplasm See e.g. SARCODINA.
ectoplasmic net See LABYRINTHULAS and THRAUSTOCHYTRIDS.
ectosymbiont An organism which lives on another organism in
a symbiotic association (SYMBIOSIS sense 1); an ectosymbiont
remains external to the cells and tissues of a host, although it may
live e.g. within the gut cavity of the host. (cf. ENDOSYMBIONT.)
Ectothiorhodospira A genus of photosynthetic bacteria originally placed in the family CHROMATIACEAE but later proposed
as type genus of a new family, Ectothiorhodospiraceae [IJSB
(1984) 34 338339]. Cells: spiral, vibrioid or rod-shaped; they
contain Bchl a or Bchl b (according to species see CHLOROPHYLLS) and various CAROTENOIDS (cell suspensions are typically
brown to brown-red). The pigments occur in lamellar intracytoplasmic membrane systems which are continuous with the
cytoplasmic membrane. Motility is mediated by a single polar
flagellum or by a polar tuft of flagella. Gas vacuoles occur in
some strains. The organisms occur typically in alkaline sulphidecontaining saline habitats; they grow optimally at pH 7.59.1
258
EHEC
E. ictaluri ). VP ve; acid (commonly with gas) from glucose;
lactose ve; phenylalanine deaminase ve; arginine dihydrolase
ve; lysine decarboxylase +ve. Vitamins and amino acids are
required for growth. Optimum temperature: 37 C (ca. 25 C for
E. ictaluri ). The organisms are usually resistant to colistin but
sensitive to other antibiotics (including penicillins); R plasmids
are rare. GC%: 5359. Type species: E. tarda.
E. anguillimortifera. Nomen dubium [Book ref. 22, pp.
488489].
E. hoshinae. Indole usually ve; MR +ve; H2 S ve (on TSI);
acid from e.g. sucrose, D-mannitol and trehalose. E. hoshinae
occurs in the intestines of animals (including mammals, fish and
reptiles).
E. ictaluri. Non-motile. Indole ve; MR ve; H2 S ve (on
TSI); no acid from sucrose, D-mannitol or trehalose. Causal agent
of ENTERIC SEPTICAEMIA in channel catfish.
E. tarda. Indole +ve; MR +ve; H2 S +ve (on TSI); usually
no acid from sucrose, D-mannitol or trehalose. A few strains
(biogroup 1) produce acid from e.g. sucrose and D-mannitol but
not from trehalose. E. tarda occurs in the intestines of animals
(including mammals, fish and reptiles). It can be an opportunist
pathogen in man, and may be a cause of diarrhoea; it can also
cause localized and generalized sepsis in fish.
[Book ref. 22, pp. 486491.]
EEE EASTERN EQUINE ENCEPHALOMYELITIS.
Eel Virus European See IPN VIRUS.
EES Ethylethane sulphonate: a mutagenic ALKYLATING AGENT.
EF (1) Elongation factor: see PROTEIN SYNTHESIS. (2) Oedema
(edema) factor: see ANTHRAX TOXIN.
efavirenz See ANTIRETROVIRAL AGENTS.
EF0 F1 H+ -ATPase See PROTON ATPASE.
effective publication See NOMENCLATURE.
efficiency of plating See EOP.
efflux mechanism (of antibiotic resistance) In some microorganisms: any of various systems (usually or always energydependent) which can mediate resistance to an ANTIBIOTIC (or
to more than one antibiotic) by extruding such agent(s) through
the cytoplasmic membrane or the cell envelope; efflux involves
a TRANSPORT SYSTEM that often consists of a complex of proteins
but which, in some cases, comprises a single protein. Efflux
transporters are classified according to their overall structure and
e.g. the homology of amino acid sequences in component proteins; some efflux systems are ABC TRANSPORTERS, while others
are found e.g. in the major facilitator superfamily (MFS) or resistancenodulationdivision (RND) superfamily. (See also MATE.)
For examples of efflux-dependent antibiotic resistance (and/or
references) see e.g. entries ABC TRANSPORTER, MACROLIDE ANTIBIOTICS, QUINOLONE ANTIBIOTICS, TETRACYCLINES.
effused-reflexed (mycol.) Refers to a sheet-like fruiting body
which lies flat against the substratum except at the edge(s), the
latter growing outwards from the substratum.
EF-G See PROTEIN SYNTHESIS (elongation).
eflornithine See SLEEPING SICKNESS.
efrapeptin A lipophilic polypeptide which binds non-covalently
to and inhibits (F0 F1 )-type PROTON ATPASES.
efrotomycin See POLYENE ANTIBIOTICS (b).
EF-Ts, EF-Tu See PROTEIN SYNTHESIS (elongation).
EGF Epidermal growth factor. (See e.g. ONCOGENE.)
egg (for cultivating viruses) See EMBRYONATED EGG.
egg-drop syndrome In general: any fall in egg production in
poultry, due e.g. to poor housing, incorrect nutrition, various
POULTRY DISEASES, etc. Egg-drop syndrome 1976 is a specific
syndrome which came into prominence in the UK and Ireland in
Ehrlichia
ehrlichiosis Any human or animal disease caused by a species
of EHRLICHIA.
Ehrlichs reagent An INDOLE TEST reagent: p-dimethylaminobenzaldehyde (1 g) is dissolved in 95100% ethanol (95 ml), and
conc. HCl (20 ml) is added; stored at 4 C in the dark.
EIA (serol.) (1) ENZYME IMMUNOASSAY. (2) ERYTHROIMMUNOASSAY.
EIAV Equine infectious anaemia virus: see SWAMP FEVER and
LENTIVIRINAE.
eicosanoids Polyunsaturated fatty acids which contain 20 carbon
atoms; examples include ARACHIDONIC ACID and LEUKOTRIENES.
EIEC Enteroinvasive Escherichia coli: strains of E. coli which
can invade and destroy epithelial cells in the ileum/colon,
causing watery diarrhoea or (bacillary) DYSENTERY. Invasiveness
is dependent on virulence genes carried by a plasmid (pInv ).
EIEC encodes a cell-surface protein analogous to the IcsA
protein of Shigella (which promotes actin-based motility within
epithelial cells: see DYSENTERY); the presence of this protein (in
EIEC and Shigella) is associated with the absence of a specific
cell-surface protease (OmpT in EIEC and SopA in Shigella)
[Mol. Microbiol. (1993) 9 459468]. EIEC produces at least
one enterotoxin: ShET2 (named after Shigella enterotoxin 2: a
similar toxin produced by S. flexneri ); this toxin is encoded by
the sen gene a (plasmid) gene formerly referred to as set2.
[Toxins produced by EIEC: MR (1996) 60 167215 (p. 188).]
At least part of the secretory (diarrhoeal) effect brought about
by invasive organisms (such as EIEC and Shigella dysenteriae)
is likely to be due to their ability to upregulate cyclooxygenase
activity in the intestinal mucosa this leading to increased
expression of PROSTAGLANDINS (such as PGE2 ) with resulting
increase in fluid secretion.
EIEC causes disease in both children and adults outbreaks
occurring e.g. in schools, hospitals and institutions. EIEC typically resembles Shigella often being non-motile, and giving
negative results in tests for lactose utilization and lysine decarboxylase.
Eijkman test An IMVEC TEST which determines the ability of an
organism to produce gas from lactose at 44 C 0.2 C; the test
is often used to confirm the presence of coliforms in a water
sample (see COLIFORM TEST) for which purpose use is made of
a medium such as lauryl tryptose lactose broth that includes an
agent which inhibits endospore-forming bacteria.
Eikenella A genus (incertae sedis) of anaerobic, facultatively
aerobic, oxidase-positive, catalase-negative, chemoorganotrophic, Gram-negative bacteria which occur e.g. in the human
mouth and intestine, and which can be opportunist pathogens.
Cells: non-motile, round-ended rods (0.30.4 1.54.0 m) or
short filaments; rods may exhibit TWITCHING MOTILITY. Growth
occurs e.g. on blood agar; haemin is required for aerobic growth
of freshly-isolated strains. Plate cultures have a bleach-like
odour. Optimum growth temperature: 3537 C. No acid is
formed from carbohydrates. Nitrate is reduced to nitrite. Urease
ve. GC%: ca. 5658. Type species: E. corrodens. [Book
ref. 22, pp. 591597.]
Eimeria
A genus of parasitic, homoxenous protozoa of the
suborder EIMERIORINA (q.v. for life cycle). Eimeria spp form
tetrasporic, dizoic oocysts (cf. e.g. ISOSPORA). No species is
known to be pathogenic in man, but many cause disease e.g.
in domestic animals (see COCCIDIOSIS).
eimeriid Of the suborder EIMERIORINA.
Eimeriina (1) A suborder of protozoa (order Eucoccida) later
incorporated together with organisms of the TOXOPLASMEA in
the suborder EIMERIORINA. (2) A suborder of protozoa (order
electron microscopy
Eucoccidiida [JP (1980) 27 3758]) equivalent to the
EIMERI-
ORINA.
electron microscopy
electron gun
anode
gun alignment coils
gun airlock
1st condenser lens
2nd condenser lens
beam tilt coils
condenser 2 aperture
objective lens
access for specimen
diffraction aperture
diffraction lens
intermediate lens
1st projector lens
2nd projector lens
binocular 12x
ELECTRON MICROSCOPY. Cross section of a transmission electron microscope (the Philips EM400). (Courtesy of N. V. Philips
Gloeilampenfabrieken, Eindhoven, Holland.)
or a replica of it.) Electron microscopy can give magnifications within the range ca. 10 to 1000000. Resolving power
depends e.g. on the nature of the specimen and on the type
of instrument used. The best resolving power is obtained with
the transmission electron microscope (see (a) below) which has
resolved a structure of ca. 1 nm periodicity in the purple membrane of Halobacterium salinarium; for non-periodic biological
specimens the best resolution may be ca. 35 nm.
Electron microscopy is used e.g. for examining viruses,
macromolecules, and the ultrastructure of cells, and for determining the intracellular locations of e.g. specific enzymes and
ions (see also IMMUNOELECTRON MICROSCOPY). Although living
electron microscopy
the electron microscope. However, biological materials can be
stained with certain heavy metal compounds which become
localized in specific regions of the specimen; this enhances the
electron-deflecting properties of those regions and/or increases
contrast between the specimen and its background.
Preparation of thin sections for the TEM. Typically, a tissue or cell initially undergoes double fixation, e.g. pre-FIXATION
with GLUTARALDEHYDE and post-fixation with OSMIUM TETROXIDE. The fixed specimen is dehydrated, e.g. by equilibration
in increasing concentrations of ethanol (or acetone) in water.
From 100% ethanol the specimen is commonly transferred to,
and equilibrated with, propylene oxide before being embedded,
i.e., impregnated with an epoxy resin (e.g. SPURRS MEDIUM)
or a methacrylate substances which polymerize and harden
without significant change in volume. (Equilibration of the specimen with propylene oxide between dehydration and embedding
is advantageous since propylene oxide is more miscible than
ethanol with epoxy resins.) The embedded specimen is then sectioned (see MICROTOME) to obtain ultrathin sections of maximum
thickness ca. 100 nm. A section is placed on a specimen holder
(grid ): a metal (usually copper) disc, 23 mm in diameter, perforated by rows of square holes each ca. 0.1 0.1 mm. Before
receiving the section the surface of the grid may be coated with a
support film: a sheet of e.g. FORMVAR or nitrocellulose 2050 nm
thick; such materials have a low, uniform electron-scattering
power. (A support film is sometimes omitted when the section
is resin-embedded; however, it is essential for a liquid specimen see e.g. negative staining below.) The support film itself
may be coated with a film of carbon (ca. 20 nm thick) which
stabilizes it and improves resolution at high magnifications. The
section, on the prepared grid, is now stained, i.e., immersed in
a solution of a heavy metal compound (e.g. uranyl acetate, lead
acetate, or a salt of phosphotungstic acid) which combines or
complexes with particular components (e.g. lipids, proteins) a
type of staining called positive staining; images subsequently
formed in the EM thus reflect the distribution of heavy metal
atoms and the groups with which they combine. (Staining is
sometimes carried out before the embedding stage by subjecting
the specimen to prolonged exposure to e.g. osmium tetroxide or
uranyl acetate; this is called in-block staining.) The section is
allowed to dry and is then ready for examination in the TEM.
Negative staining (negative contrast) is used to reveal the
outlines and surface contours of particulate specimens (e.g.
macromolecules, viruses, bacteria). Essentially, the particles are
immersed in a thin film of electron-opaque stain on a prepared
grid; the stain penetrates the interstices of each particle and
forms a thin background layer but usually does not permeate
the particles themselves. Electrons are more readily transmitted
through those regions occupied by the (relatively) electrontransparent particles, so that in the image these regions appear
bright against a dark background; the presence of stain in surface
hollows and grooves indicates surface topography. For example,
the TOBACCO MOSAIC VIRUS virion appears as a light rod in which
a dark, central, axial line indicates the presence of stain in
the hollow core. To examine bacterial morphology, one drop
of (fixed or unfixed) bacterial suspension is left on a prepared
grid for one or more minutes (determined by trial and error)
so that cells adhere to the surface; most of the drop is then
drawn off with the edge of a filter paper. One drop of stain (e.g.
2% aqueous phosphotungstic acid or 2% aqueous ammonium
molybdate) is then placed on the grid; after 3060 seconds this
is drawn off, as before. The fine film on the grid is left to dry
and is examined in the TEM. (Alternatively, stain and suspension
can be mixed, and the stained suspension applied to the grid.)
Shadowing (shadow-casting) is used e.g. to study the morphology and/or dimensions of e.g. viruses and bacteria, and is
also involved in the KLEINSCHMIDT MONOLAYER TECHNIQUE for
examining nucleic acids. Essentially, the particles (e.g. viruses)
on a prepared grid are exposed to a point source of the vapour
of a heavy metal; the point source is so placed that metal is
deposited on only one side of each particle leaving a nonmetallized (electron-transparent) shadow on the remainder of
the particle and on that part of the support film shielded (by the
particle) from the vapour. The image of a shadowed particle can
give information on the shape and size of the particle; its size
can be calculated from the length of the shadow and the angle
at which the metal vapour was incident on the particle.
Replicas of e.g. a freeze-etched specimen (see FREEZEETCHING) may be examined in the TEM. Essentially, this
involves shadowing the surface of the frozen specimen with a
heavy metal under vacuum; commonly, shadowing is effected
at an angle of ca. 30 with a mixture of platinum and carbon vapours. Shadowing throws into relief the features of an
irregular surface. Areas protected from the vapour remain nonmetallized and are therefore structurally weak; the primary
replica is therefore strengthened by deposition of a layer of
carbon from a vapour source placed directly above the specimen. The replica is cleaned by digesting away the specimen
with strong oxidizing and hydrolysing agents (e.g. bleach, sulphuric acid, chromic acid). The replica is mounted on a grid and
examined in the TEM.
The transmission electron microscope (TEM ). A typical TEM
is shown in the figure. The electron beam originates at a heated
metal filament in the electron gun. The electrons are accelerated
through a hole in the anode and pass down through the axis of the
instrument; acceleration is caused by a large potential difference
(accelerating voltage) maintained between the anode (at earth
or zero potential) and the filament (commonly 100 kV to
500 kV). The accelerating voltage determines the wavelength
of the electron beam which, in turn, determines the resolving
power; in general, higher accelerating voltages give better
resolving power. (Some specimens can be damaged more than
others by high accelerating voltages; resolving power is therefore
partly determined by the nature of the specimen.) The various
magnetic lenses each consist basically of a soft-iron reel on
which are wound many turns of copper wire; current passing
through the wire generates a magnetic field which controls the
electron beam passing axially through the lens. The specimen,
on a grid, is placed in the path of the electron beam; electrons
which pass through the specimen are focused to form an image
on a screen consisting of a metal plate coated with a fluorescent
material. During operation, the interior of the tube-like body
(column) of the microscope must be evacuated to prevent e.g.
deflection and scattering of the electrons by molecules of gas;
pressure in the column is usually less than ca. 6.5 105 Pa
(5 107 torr; 0.5 nm Hg).
(b) Scanning electron microscopy is used to examine the
surface of a specimen. The specimen is scanned by an electron
beam which moves in a zig-zag raster; a second electron
beam synchronously scans a cathode ray tube (CRT) with a
similar raster. Electrons which are secondarily emitted from the
specimen are collected and used to control the intensity of the
beam in the CRT. Since the secondarily emitted electrons vary in
quantity from point to point on the specimens surface (according
to surface topography) the electron beam in the CRT will be
continually modulated as the specimen is scanned; hence, the
CRT screen will display a pattern of bright and less-bright spots
corresponding to the surface topography of the specimen.
263
The scanning electron microscope (SEM) can give magnifications of ca. 10 to 100000; for biological specimens it is
commonly used at magnifications below ca. 10000. Resolution is usually ca. 1020 nm. The SEM provides a great depth
of field, thus giving valuable three-dimensional images.
Preparation of specimens for the SEM. Completely untreated
specimens have been examined in the SEM. However, specimens (particularly plant material) are often given the following
sequence of treatments. (i) Fixation and dehydration as for
TEM thin sections described above. (ii) Drying (removal of all
liquid); this is sometimes achieved by FREEZE-DRYING (simultaneous dehydration and drying) but more usually by CRITICAL POINT
DRYING. (iii) Attachment of the specimen to a metal (often aluminium) specimen holder (stub) by means of a glue (e.g. SILVER
DAG) which conducts both heat and electricity. (iv) Coating of
the specimen, under vacuum, with carbon and/or metal usually
by SPUTTER-COATING; this prevents thermal and electrical buildup on the specimen when it is placed in the electron beam
(thus avoiding image distortion and damage to the specimen)
and enhances secondary electron emission. (As an alternative to
coating, the specimen may be thoroughly impregnated, before
dehydration, with e.g. osmium tetroxide.) The specimen is then
ready for the SEM.
Replicas of a specimen may be made e.g. if repeated
observations are to be made of the same specimen. Essentially,
fluid plastic or latex is poured over the specimen and allowed
to harden. This gives a negative replica which is peeled off and
lined with a suitable material that hardens to form the positive
replica; the latter is sputter-coated and examined in the SEM.
(c) Scanning transmission electron microscopy. In the scanning transmission electron microscope (STEM) electrons pass
through the specimen, and the energies of the emergent electrons are measured in an analyser. The pattern of energies of the
emergent electrons is used to construct an image of the specimen.
The resolving power of the STEM can be similar to that of the
TEM. [Introduction to STEM: JUR (1984) 88 94104; imaging
biological structures: JUR (1984) 88 105120, 177206.]
(d) Low temperature electron microscopy (cryoelectron microscopy). A type of electron microscopy in which very small
specimens are cooled rapidly to very low temperatures, without prior dehydration, such that the water in the specimen forms
a glass-like solid without undergoing crystallization a phenomenon called vitrification [review: TIBS (1985) 10 143146].
(e) Three-dimensional electron microscopy. A procedure intended for three-dimensional examination of biological structures at atomic resolution. [ARBB (1981) 10 563592.]
electron paramagnetic resonance Syn. ELECTRON SPIN RESONANCE.
electron spin resonance (ESR; electron paramagnetic resonance,
EPR) The absorption and consequent emission of electromagnetic radiation by unpaired electrons in certain types of atom in
the presence of a strong magnetic field; in general principle ESR
resembles NUCLEAR MAGNETIC RESONANCE (q.v.).
Molecules in which atom(s) contain unpaired, ESR-detectable
electrons are paramagnetic and are commonly called free radicals. In biological materials free radicals are produced during
many types of metabolic process but they are typically shortlived; however, a stable, paramagnetic probe (spin label ) can be
introduced into an experimental system e.g. by biosynthetic
incorporation or by covalent linking to specific compounds. Most
spin labels contain the nitroxide (NO) group; they include derivatives of fatty acids, of the steroids androstane and cholestane, and
of 2,2,6,6-tetramethylpiperidine. (In some studies on membrane
264
fumarate
+
Complex II
NAD
fumarate
FAD
Fe-S centres
b -type cyt
Complex I
NADH
UQ
site 1
Complex IV
Complex III
a3
Cu Cu
site 2
NAD
1
2 O2
+ 2H+
H2O
site 3
proton
motive force
mH+
NAD + NADPH
ion transport
transhydrogenase
+
NADH + NADP
proton ATPase
'Complex V'
proton PPase
ATP + H2O
PPi
+ H2O
ADP + Pi
2Pi
ELECTRON TRANSPORT CHAIN. A scheme for electron transport in an animal-type mitochondrion, showing electron transfer from NADH
and/or succinate to the terminal electron acceptor, oxygen. (Electron transport is believed to be similar in the mitochondria of many types
of microorganism.) Sites 1, 2 and 3 indicate sites of transmembrane proton translocation during electron flow. Thick lines indicate energy
conversion (or regulation in the case of transhydrogenation). FMN = flavin mononucleotide; FeS centre = ironsulphur centre; FAD = flavin
adenine dinucleotide; b562 , c1 etc = cytochromes; UQ = ubiquinone; proton PPase = proton pyrophosphatase.
electroneutral transport
electrophoretic transport Transport of a charged species across
an energy-transducing membrane in response to a pre-existing
transmembrane electrical potential difference. (cf. ELECTRICAL
TRANSPORT.)
electroporation An in vitro method for increasing the efficiency
of TRANSFORMATION. Essentially, a mixture of cells and e.g.
plasmids is exposed to an electric field (up to 16 kV/cm) for
a fraction of a second; the mechanism of uptake is unknown,
but the frequency of transformation varies linearly with the
concentration of DNA over a wide range of values, and the
efficiency of transformation varies with cell concentration.
[Electroporation in Helicobacter pylori: AEM (1997) 63
48664871; in Escherichia coli: NAR (1999) 27 910911.]
Electrocompetent (electroporation-competent) cells with
high-level transformation efficiency are available commercially.
The electrocompetent cells marketed by Stratagene (ElectroTenBlue ) are electroporated at 1.7 kV and 600 ohms resistance.
ElectroTen-Blue See ELECTROPORATION.
electro-transfection Electrically-assisted TRANSFECTION; thus,
e.g. tobacco protoplasts have been transfected with RNA from
the tobacco mosaic virus under the influence of 50-sec pulses
of DC current at 550800 V/cm [JGV (1986) 67 20372042].
(cf. ELECTROFUSION.)
Elek plate An in vitro method for detecting the formation of
a diffusible toxin by a given strain of microorganism, e.g.
Corynebacterium diphtheriae. A plate of suitable medium is
inoculated, in a straight line, with the strain under test; the streak
is then overlaid, perpendicularly, with a strip of paper which
has been impregnated with relevant antitoxin. After incubation
(2448 hours), toxin production is indicated by the development
of lines of whitish precipitate which approximately bisect each
of the four right angles formed by the paper strip and the line of
microbial growth; the precipitate results from the combination
of toxin and antitoxin following their diffusion from the line
of growth and paper strip, respectively. Non-specific lines of
precipitate may be formed, so that known negative and positive
strains must be used as controls.
Several unknown strains, and the controls, may be examined
on a standard-size Petri dish.
In a modified form of the test, an antitoxin-impregnated disc
is placed at the centre of the plate, and the test strain(s), together
with positive and negative controls, are inoculated in a circular
pattern at a fixed radius; this form of test can be read after 16
hours [JCM (1997) 35 495498].
Diphtheria toxin can also be detected directly from clinical
specimens by a PCR-based method which detects the A and
B subunits of the toxin; a result can be available within hours
of collecting the specimen. This assay is used in the Diphtheria
Laboratory at the Centers for Disease Control in the USA [JCM
(1997) 35 16511655].
elementary body (EB) (1) See CHLAMYDIA. (2) An archaic name
for a virion.
ELISA (enzyme-linked immunosorbent assay) A highly sensitive IMMUNOASSAY for specific antibodies or antigens. For the
assay of specific antibodies, the antiserum (or other test material)
is allowed to react with homologous antigens which have been
adsorbed e.g. to the inner surface of a plastic tube; uncombined
antibodies are removed by washing. Antibodies which have combined with the immobilized antigens are then detected by treating
the test system with a conjugate (see CONJUGATION sense 2) consisting of anti-immunoglobulin antibodies each covalently linked
to an enzyme of a particular type; the test system is washed free
of any uncombined conjugate and examined for bound enzyme
embryonated egg
K2 HPO4 (0.2%); eosin Y (0.04%); methylene blue (0.0065%);
agar (ca. 1.5%). Final pH: ca. 7.2. Colonies of Escherichia
coli usually have dark centres and a greenish metallic sheen,
those of Enterobacter aerogenes are usually mucoid, brownish
in the centre, and only occasionally show a metallic sheen, while
those of Salmonella and Shigella are usually colourless and
translucent.
EmbdenMeyerhofParnas pathway (EMP pathway; EmbdenMeyerhof pathway; hexose bisphosphate pathway; glycolysis)
A sequence of reactions in which glucose is broken down to
pyruvate . The EMP pathway occurs in a wide range of organisms, both prokaryotic and eukaryotic, and can operate under
both aerobic and anaerobic conditions. By this pathway one
molecule of glucose yields two molecules each of pyruvate and
NADH and two (net) of ATP (from SUBSTRATE-LEVEL PHOSPHORYLATION); if glucose 6-phosphate is derived from GLYCOGEN,
the net yield of ATP is 3 molecules. [See Appendix I(a).] In
respiratory modes of metabolism (see RESPIRATION) the pyruvate is commonly converted to acetyl-CoA which enters the TCA
CYCLE; NADH is oxidized via a respiratory chain (see ELECTRON
TRANSPORT CHAIN). In fermentative modes (see FERMENTATION)
the fate of pyruvate depends on species and/or conditions, but
must always involve regeneration of NAD+ from NADH by
reduction of an endogenous substrate (see e.g. ALCOHOLIC FERMENTATION, HOMOLACTIC FERMENTATION, and Appendix III).
The initial step of the EMP pathway, the formation of glucose 6-phosphate from glucose, is catalysed by hexokinase in
e.g. yeasts and some bacteria, while in other bacteria (e.g.
enterobacteria, streptococci) glucose is phosphorylated during
its uptake by a PTS (q.v.). Phosphofructokinase is a key enzyme
in the EMP pathway, and the presence of this enzyme in an
organism is generally taken as evidence that the EMP pathway
occurs in that organism. In yeasts (and e.g. mammals) phosphofructokinase is inhibited by high levels of ATP and citrate, and
is stimulated by high levels of AMP; in e.g. Escherichia coli
phosphofructokinase is inhibited by phosphoenolpyruvate (but
not by citrate), and is stimulated by ADP and GDP (but not by
AMP). (See also ADENYLATE ENERGY CHARGE.) (In certain organisms fructose 6-phosphate is phosphorylated by a pyrophosphate:phosphofructose dikinase see PYROPHOSPHATE.)
The EMP pathway functions not only in energy-yielding
metabolism but also in supplying intermediates for biosynthesis: e.g., dihydroxyacetone phosphate can be reduced to glycerol
phosphate for use in the biosynthesis of lipids; phosphoenolpyruvate may be drawn off for aromatic amino acid biosynthesis
[Appendix IV(f)], 3-phosphoglycerate for cysteine, glycine and
serine biosynthesis [Appendix IV(c)], and pyruvate for alanine,
leucine and valine biosynthesis [Appendix IV(b)]. (See also GLUCONEOGENESIS.)
(See also ENTNERDOUDOROFF PATHWAY; GLYCOSOMES; HEXOSE
MONOPHOSPHATE PATHWAY; METHYLGLYOXAL BYPASS.)
The terms EMP pathway and glycolysis are often used for
the complete pathway for glucose degradation: e.g. glucose
lactate (i.e., HOMOLACTIC FERMENTATION) or glucose ethanol
(i.e., ALCOHOLIC FERMENTATION).
embedding See MICROTOME and ELECTRON MICROSCOPY.
embryonated egg (embryonating egg) An egg (usually a hens or
ducks egg) which contains a live, developing embryo. Such eggs
are used in virology e.g. for the identification, culture, and/or
assay of certain viruses (see e.g. POCK sense 2), and as a source
of cells for TISSUE CULTURE.
An embryonated egg is prepared by incubating a fertile egg
in a humid atmosphere for ca. 514 days at e.g. 3739 C the
EMCV
growth is transferred to, and mixed with, a drop of the liquid on
a slide.
(2) The formation of an emulsion, i.e., a suspension of droplets
of one liquid in another with which it is non-miscible (e.g.
oil in water). Substances which stabilize emulsions are called
emulsifying agents. (See also BIOSURFACTANTS.)
enanthem A rash on a mucous membrane (cf. EXANTHEM).
enation (plant pathol.) A localized proliferation of leaf tissue
caused e.g. by viral infection.
encapsidation During virion assembly: the process in which
nucleic acid becomes incorporated in the viral capsid or e.g.
in certain bacteriophages in a head/capsid precursor.
encephalitis Inflammation of the brain; it is often accompanied
by inflammation of the brain meninges (encephalomeningitis,
MENINGOENCEPHALITIS) or the spinal cord (encephalomyelitis) or
both (meningoencephalomyelitis). Symptoms range from mild
(fever, headache, malaise, myalgia, stiffness of the neck and
back) to severe (irritability or somnolence, coma, death). Causes
of encephalitis are many and varied. Toxic encephalitis results
from severe toxaemia early in the course of an acute infectious
disease. Post-infective encephalitis occurs after the onset of
certain diseases (e.g. CHICKENPOX, MEASLES, MUMPS, WHOOPING
COUGH). Post-vaccinal encephalitis may follow active immunization against e.g. rabies, smallpox, whooping cough, yellow fever.
Viral encephalitis may be caused by any of a range of viruses:
see e.g. B VIRUS; CALIFORNIA ENCEPHALITIS; EASTERN EQUINE
ENCEPHALOMYELITIS; HERPES SIMPLEX; JAPANESE B ENCEPHALITIS;
POWASSAN ENCEPHALITIS; RUSSIAN SPRINGSUMMER ENCEPHALITIS;
ST LOUIS ENCEPHALITIS; SUBACUTE SCLEROSING PANENCEPHALITIS; VENEZUELAN EQUINE ENCEPHALOMYELITIS; WESTERN EQUINE
ENCEPHALOMYELITIS. Amoebic encephalitis may involve e.g. certain species of ACANTHAMOEBA or NAEGLERIA or BALAMUTHIA
MANDRILLARIS.
(See also MENINGITIS, TALFAN DISEASE, TESCHEN DISEASE;
TRANSMISSIBLE SPONGIFORM ENCEPHALOPATHIES.)
Encephalitozoon
A genus of protozoa (class MICROSPOREA).
E. cuniculi (= Nosema cuniculi) is parasitic (but generally nonpathogenic) in rodents and other animals, and has been recorded
as the cause of a case of human encephalitis; it has also
been isolated from eye, intestine, kidney, liver and peritoneum.
[Mechanism of resistance to E. cuniculi in mice: J. Imm. (1984)
133 27122719.] The spores of E. cuniculi (ca. 2.5 1.5 m)
can be isolated from the urine of infected animals.
E. intestinalis can cause travellers diarrhoea [PCR-based
identification of E. intestinalis: JCM (1998) 36 3740].
encephalomeningitis See ENCEPHALITIS.
encephalomyelitis See ENCEPHALITIS.
encephalomyocarditis virus (murine) See CARDIOVIRUS.
encystment The formation of a CYST.
end-point dilution assay (virol.) A method of quantifying a
given type of virus in a given sample, i.e., measuring the infectivity of that virus in the sample. In this method, infectivity is
measured by determining the extent to which the sample must
be diluted in order that a given volume of the dilution corresponds to the LD50 , TCID50 or (more generally) the ED50 of
the virus. Initially, log (or semi-log) dilutions of the sample
are prepared. Each dilution is then examined, individually, by
inoculating each of a number of similar test units with a fixed
volume (dose) of that dilution; test units may be e.g. susceptible
laboratory animals or tissue cultures which undergo detectable
forms of degeneration when infected with the virus. After incubation, each test unit is examined. Animals or cultures inoculated
with a dose from the lower dilutions (i.e. higher concentrations
endocytosis
as the highest dilution which exhibits agglutination in the test
system. (See also TITRE.)
end-product efflux The outflow, from a growing cell, of the
end products of metabolism; in some cases such efflux involves
end-productproton SYMPORT (e.g. lactateproton symport) capable of generating, or augmenting, a proton motive force (see
CHEMIOSMOSIS). Such a mechanism for energy conversion may
be particularly important e.g. in at least some obligately fermentative bacteria. In these organisms (which lack a respiratory
chain) the pmf required e.g. for certain TRANSPORT SYSTEMS can
be generated by ATP hydrolysis at a PROTON ATPASE though
this process is likely to consume much of the ATP generated by
substrate-level phosphorylation; pmf generation by end-product
efflux has been reported e.g. in Lactococcus lactis (formerly
Streptococcus cremoris) [AvL (1984) 50 545555; JB (1985)
162 383390].
Endamoeba
A genus of cyst-forming amoebae (order AMOEBIDA) parasitic in the gut of invertebrates (e.g. E. blattae in
cockroaches). The nucleus lacks a karyosome.
endemic (1) Of a disease: commonly or constantly present in
a given location or geographical region; typically, a relatively
low proportion of the local population exhibits clinical signs
of the disease. (2) Constantly present in a given location or
geographical region.
Endemosarca A genus of endoparasitic, plasmodium-forming
eukaryotic organisms which are parasitic in ciliates (Colpoda
spp); they appear to be related to members of the PLASMODIOPHOROMYCETES. [Book ref. 147, pp. 203206.]
endergonic reaction Any reaction requiring an uptake of energy.
(cf. EXERGONIC REACTION.)
endobiotic Living within a host organism.
endocarditis Inflammation of the endocardium, i.e. the tissue
lining the cavities of the heart.
Infective (infectious) endocarditis may be due to infection
by any of a range of microorganisms e.g. Haemophilus sp,
Staphylococcus aureus, S. epidermidis (especially in patients
with prosthetic heart valves), Enterococcus faecalis, viridans
streptococci (see also NUTRITIONALLY VARIANT STREPTOCOCCI),
Neisseria gonorrhoeae, Candida, Aspergillus, Histoplasma.
Infrequently, the causal agent is one of the more recently
described species of coagulase-negative staphylococci: S. lugdunensis [RMM (1995) 6 94100]. (See also CARDIOBACTERIUM.)
Infective endocarditis may be acute or subacute; S. aureus
may cause either acute or subacute endocarditis. Infection occurs
via the bloodstream. Organisms may gain access to the bloodstream e.g. during dental treatment (e.g. oral viridans streptococci), catheterization or insertion of an intrauterine contraceptive device (e.g. faecal streptococci), intravenous injection (e.g.
staphylococci) etc.
Symptoms: e.g. fever, malaise, heart murmurs, weight loss,
clubbing of fingertips, embolism; late symptoms of subacute
bacterial endocarditis (SBE) include vasculitis, petechial rash,
and (almost pathognomonic) small, tender, often bluish swellings
on the skin (Oslers nodes). Damage to heart valves may lead
to heart failure.
Endocarditis may occur as a complication of other infectious diseases e.g. Q FEVER, SYPHILIS, TUBERCULOSIS. (See also
RHEUMATIC FEVER.)
Endocarpon See VERRUCARIALES.
endocellulase See CELLULASES.
endocyst See CYST (b).
endocytobiosis Syn. CYTOBIOSIS.
endocytosis The ingestion of materials, by a cell, by PHAGOCYTOSIS and/or PINOCYTOSIS.
of virus) may react positively in every case; of those inoculated with a dose from the higher dilutions some may react
positively while others are unaffected. The important dilution
is that which corresponds to the ED50 ; such a 50% end point
is not always obtained experimentally, but it may be calculated
from the experimental data provided that some test units have
given a negative reaction. The 50% end-point dilution may be
calculated by the ReedMuench method or the Karber method;
however, these methods can be used only if the dilutions are in
a regular logarithmic sequence, and only if a similar number of
test units is used for each dilution. Examples of the use of these
methods are given below with reference to the specimen data in
the accompanying table.
END-POINT DILUTION ASSAY: specimen data
Column A: Column B: Column C: Column D: Column E:
dilution of mortalities in cumulative cumulative C/(C + D)%
virus
5 test animals mortalities survivors
106
105
104
103
0/5
2/5
4/5
5/5
0
2
6
11
9
4
1
0
0
33.3
85.7
100
50 33.3
85.7 33.3
The logarithm of the 50% end point is thus 104.68 ; since the
antilog of 4.68 is ca. 48000 a dose from the 1/48000 dilution of
the sample will contain the LD50 .
Karber method. Substitutions are made in the following
equation:
log10 50% end point = L1 L(S 0.5)
in which L1 = logarithm of lowest dilution tested; L = log
interval between dilutions; S = sum of the proportion of positive
reactions at each dilution; 0.5 is a constant. In the accompanying
table, S = 0 + 0.4 + 0.8 + 1.0 = 2.2; hence, the required value
is 104.7 .
An estimate of the number of infectious virions in the original
(undiluted) sample can be derived from the expression:
n = loge (1 p)
in which n = average number of infectious virions per dose;
p = proportion of positive reactions in the test units inoculated
from a given dilution; e = 2.7183. The value of n (calculated
for one of the dilutions) multiplied by the dilution factor gives
an estimate of the viral titre of the sample; such an estimate is
less reliable than that made from a PLAQUE ASSAY.
end-point titration (serol.) A method of assaying the concentration of a specific antibody or antigen, in a given sample, by
determining the highest dilution of the sample which gives a
reaction regarded as positive under the conditions of the test. For
example, in an agglutination test the end point may be regarded
269
endodyogeny
endolysin is to lyse the host cells envelope to release phage
progeny. In many or all cases, endolysins (which lack a signal
sequence) are enabled to cross the cytoplasmic membrane (to
reach peptidoglycan) by means of a LYSIS PROTEIN.
endometritis Inflammation of the endometrium. In humans and
animals it may result from infection of the endometrium
by various opportunist pathogens (e.g. Klebsiella pneumoniae,
Pseudomonas aeruginosa, group A streptococci). (See also
CONTAGIOUS EQUINE METRITIS.)
endomitosis Chromosome replication without nuclear division.
(cf. MITOSIS.)
Endomyces See ENDOMYCETALES.
Endomycetaceae See ENDOMYCETALES.
Endomycetales An order of mainly saprotrophic fungi of the
ASCOMYCOTINA; the organisms include both unicellular and
dimorphic species. Ascocarps are not formed. Asci (which
develop from individual cells, or from cells within hyphae):
prototunicate, cylindrical to spheroidal. Families: Dipodascaceae
(genera: e.g. Dipodascus, Phialoascus), Endomycetaceae (formerly Ascoideaceae; genera: e.g. Cephaloascus, Endomyces),
METSCHNIKOWIACEAE, SACCHAROMYCETACEAE.
Endomycopsis
An obsolete fungal genus; species are now
included e.g. in SACCHAROMYCOPSIS.
endomycorrhiza See MYCORRHIZA.
endonuclease A NUCLEASE which cleaves phosphodiester bonds
within a nucleic acid strand. See also RESTRICTION ENDONUCLEASE; cf. EXONUCLEASE.
endonuclease III See BASE EXCISION REPAIR.
endonuclease S1 (nuclease S1 , endonuclease S1, etc) A zinccontaining ENDONUCLEASE, first obtained from Aspergillus
oryzae, which specifically cleaves ssDNA and ssRNA to yield
mainly 5 -nucleoside monophosphates. It can cleave local regions
of ssDNA in a dsDNA molecule.
endonucleobiosis SYMBIOSIS in which one symbiont occurs
within the nucleus of the other (see e.g. HOLOSPORA). [Endonucleobiosis in ciliates: Int. Rev. Cytol. (1986) 102 169213.]
endoparasite See PARASITE.
endoparasitic slime moulds See PLASMODIOPHOROMYCETES.
endopectate lyase See PECTIC ENZYMES.
endopectin lyase See PECTIC ENZYMES.
endopeptidase See PROTEASES.
endoperidium See LYCOPERDALES.
endoperoxide synthase Syn. cyclo-oxygenase (see PROSTAGLANDINS).
endophloeodal (endophloedal; hypophloeodal) Growing within
bark (cf. CORTICOLOUS).
Endophyllum See UREDINIOMYCETES.
endophyte (1) An organism parasitic partly or wholly within a
plant.
(2) Any of certain fungi parasitic in grasses; such fungi
include e.g. Epichloe typhina. Infection with certain endophytes
can have beneficial and harmful effects on the growth and
utilization of pasture grasses. [Artificial infection of grasses with
endophytes: Ann. Appl. Biol. (1985) 107 1724.]
endoplasm See e.g. SARCODINA.
endoplasmic reticulum (ER) Within a eukaryotic cell: a system
of membranes which ramifies through the cytoplasmic region
and forms the limiting boundaries of compartments and channels
whose lumina are completely isolated from the cytoplasm;
the ER membrane is a protein-containing lipid bilayer. In
some regions the outer surface of the ER membrane (i.e., that
surface in contact with the cytoplasm) bears many ribosomes;
such regions are called rough ER (RER), while those regions
endodyogeny Asexual reproduction (found e.g. in Chlamydomonas, Sarcocystis, Toxoplasma) in which two daughter cells
form within the parent cell (which is destroyed during the process).
endoenzyme An ENZYME which cleaves bonds within a polymer
chain: see e.g. a-AMYLASES. (cf. EXOENZYME.)
endoflagellum See SPIROCHAETALES.
endogenote See MEROZYGOTE.
endogenous infection Infection by an organism which is part
of the normal body microflora. (See e.g. CANDIDIASIS; cf.
OPPORTUNIST PATHOGENS.)
endogenous retrovirus A retrovirus (see RETROVIRIDAE) which
occurs, in provirus form, in the DNA of all normal cells of
the host species or strain, and which is transmitted genetically
via the germ line from one generation to the next. Endogenous
retroviruses have been detected in a very wide range of vertebrates (including man [see e.g. JV (1986) 58 955959]); they are
believed to have arisen by exogenous infection of germ line tissue in the (recent or possibly ancient) ancestors of the host. Many
endogenous retroviruses are related to horizontally transmissible
EXOGENOUS RETROVIRUSES. Most endogenous proviruses are transcriptionally silent. Many appear to be defective, but some can
be activated under certain conditions (e.g. by host hormones,
or by exposure to radiation or certain chemicals e.g. BUdR),
when expression may range from transcription of selected virus
genes to production of complete virus particles which may be
infectious or non-infectious, ECOTROPIC or XENOTROPIC, etc. (See
also MOUSE MAMMARY TUMOUR VIRUS.)
endoglucanase See e.g. CELLULASES.
Endogonales An order of fungi (class ZYGOMYCETES) which form
zygospores and in which asexual reproduction involves the
formation of chlamydospores, azygospores or sporangiospores.
Many species are involved in MYCORRHIZA formation (see
also RHIZOSPHERE). Genera include Acaulospora, Endogone,
Gigaspora, Glomus and Sclerocystis.
Endogone See ENDOGONALES.
Endolimax
A genus of protozoa (order AMOEBIDA) parasitic
in vertebrates and invertebrates. E. nana occurs in the human
large intestine; it is non-pathogenic. Trophozoites of E. nana
(ca. 612 m diam.) contain numerous vacuoles and form
blunt pseudopodia slowly; the single nucleus lacks peripheral
chromatin but contains a large, eccentrically located karyosome.
Cysts are usually ovoid, 48 816 m, and contain four
nuclei when mature; chromatoid bodies are usually absent.
endolithic Growing within rock, stone etc (cf. SAXICOLOUS).
For example, certain cyanobacteria, lichens and microfungi
can grow endolithically in environments too extreme (e.g. too
hot or too cold) to allow normal EPILITHIC growth. Endolithic
organisms (endoliths) have been categorized into three principal
groups: chasmoendoliths, which colonize fissures and cracks
in the rock; cryptoendoliths, which colonize structural cavities
within porous rocks; and euendoliths, which actively penetrate
the rock (e.g. by releasing substances which dissolve the
rock). [J. Sed. Pet. (1981) 51 475478.] In e.g. hot desert
regions, cyanobacteria and other bacteria are generally the
dominant cryptoendoliths, while in the dry desert valleys of
the Antarctic chasmoendolithic and cryptoendolithic lichens
(mainly Acarospora, Buellia, Lecanora and Lecidea spp) are
dominant [Science (1982) 215 10451053]. These organisms
generally inhabit a narrow zone below the rock surface, any
fruiting structures being formed at the surface. (See also e.g.
ARTHOPYRENIA; LECANORA; OSTREOBIUM.)
endolysin A PEPTIDOGLYCAN-degrading enzyme (e.g. LYSOZYME)
encoded by many types of bacteriophage; the function of an
270
endospore stains
are themselves regulated at the level of transcription by factors
dependent on the cells physiological state. Thus, whether or not
sporulation occurs appears to depend on the opposing influences
of kinases (promoting sporulation) and phosphatases (inhibiting
sporulation) [TIM (1998) 6 366370].
During the process of sporulation, gene expression is regulated, at least partly, at the level of transcription relevant
genes being transcribed in a specific temporal sequence; such
regulation involves certain SIGMA FACTORS (see figure).
Elucidation of the mechanism of sporulation has been assisted
by the isolation of various mutants, each blocked at a specific
stage of the process. Such spo mutants are designated according
to the stage beyond which endospore development does not
progress in the mutant cell; mutations which affect the same
stage but which occur at different loci are designated A, B etc.
Various mutations at spo0 loci prevent the development of the
asymmetrical septum. No stage I mutants have been detected.
In general, spo mutations have little or no effect on vegetative
growth.
The figure (part b) outlines the stages of development of an
endospore.
Dormancy. Freshly formed endospores usually enter a period
of DORMANCY in which little or no metabolic activity can be
detected.
Activation. This is a commonly reversible process in which
a dormant endospore prepares for subsequent germination and
differentiation into a vegetative cell; it appears to involve
changes in the configuration of the endospores macromolecules presumably early steps in the mobilization of
metabolic potential. Activation may be brought about e.g. by
a short period of sublethal heating, by ageing, or by subjecting
the endospores to low pH or to certain chemicals. The mode of
activation in nature is apparently unknown.
Germination is an irreversible process in which an endospore
becomes metabolically active. The process is largely degradative; it involves e.g. hydrolysis and de-polymerization of certain
constituents of the endospore, and is characterized by the release
of dipicolinic acid, calcium ions, and the breakdown products of
cortical peptidoglycan. Concurrently there is a loss of resistance
to heat, and a fall in optical density.
Germination requires, or is promoted by, certain substances
(germinants) such as L-alanine, L-proline, certain sugars (e.g.
glucose), ions (e.g. potassium, calcium, manganese, strontium),
and surfactants; a given germinant may be effective for the
endospores of some species but not for those of others. Germination is also affected by factors such as pH, and may be
promoted by mechanical damage to the spore wall.
Certain substances (e.g. D-alanine, sodium bicarbonate) inhibit
germination of the endospores of certain species.
Outgrowth is the process in which a vegetative cell develops
from a germinated endospore. (See also MICROCYCLE SPORULATION.)
(b) (cyanobacteriol.) See BAEOCYTE.
(c) (mycol.) See e.g. COCCIDIOIDES, OOSPORIDIUM, RHINOSPORIDIUM, SARCINOSPORON, TRICHOSPORON.
(2) (mycol.) (syn. endosporium) The innermost layer of a
fungal spore wall.
endospore stains Bacterial endospores stain poorly (or not at all)
with simple staining procedures in the cold. They can be stained
e.g. by a modified form of ZIEHLNEELSENS STAIN in which
ethanol (only) is used for decolorization. In another method
(SchaefferFulton stain) an air-dried, heat-fixed smear is flooded
with 0.5% (w/v) aqueous malachite green and heated to nearboiling for 5 min; the smear is then washed in running water,
Signal
Signal
KinA
KinB
P
ATP
ATP
ADP
ADP
Spo0F
spollD
Spo0B
spollG ( E)
P
spo0A
spollA ( F)
Spo0A~P
spo0F
spollE
Spo0E
spo0H ( H )
abrB
hpr
sinl
sinR
ENDOSPORE (a): simplified scheme for the regulation of gene expression during the initiation of sporulation in Bacillus subtilis.
The mechanism for initiating sporulation appears to recognize both external (environmental) and internal (intracellular) signals. These signals
are believed to promote ATP-dependent autophosphorylation of certain kinases shown in the diagram as KinA and KinB. The kinases transfer
P ) to a sequence of proteins: Spo0F Spo0B Spo0A (the so-called phosphorelay) [COGD (1993) 3 203212;
phosphate (symbol
JCBiochem. (1993) 51 5561]. The intracellular concentration of the phosphorylated form of Spo0A (Spo0AP) appears to be the key factor
in initiating sporulation; this protein is a transcription factor which promotes the expression of certain sporulation-specific genes (dashed box,
centre right) and also regulates genes shown in the two other dashed boxes.
;
+ indicates that the expression of a given gene is promoted. Control
In the diagram, inhibitory influences are indicated by the symbol
is commonly exercised at the level of transcription.
Spo0AP promotes the expression of genes spo0F and spo0A (dashed box, left) by a positive feedback loop [Mol. Microbiol. (1993) 7
967974]. Also, by repressing abrB (lower dashed box), Spo0AP promotes the expression of spo0H whose product (the SIGMA FACTOR sH )
is required e.g. for the transcription of spo0F and spo0A. sH is produced at low level during vegetative growth, but its production is greatly
enhanced following the initiation of sporulation. During sporulation, sH is needed for transcription of the ftsZ gene (see FtsZ in CELL CYCLE) from
a special promoter, p2, which is distinct from the ftsZ promoter used during exponential growth; FtsZ is required for the formation of the
asymmetrical septum.
Spo0E is a negative regulator of the phosphorelay [PNAS (1994) 91 17561760]; it is an enzyme which de-phosphorylates (and thus
inactivates) Spo0AP and which may therefore help to prevent the initiation of sporulation until the cumulative effect of the various
(extracellular and intracellular) signals dictates that sporulation is necessary.
Development of the asymmetrical septum (i.e. at a polar rather than a mid-cell location) initially involves the formation of a mid-cell Z ring
(see CELL CYCLE) i.e. as occurs during vegetative cell division. Later, this Z ring develops into a helical structure that extends into both poles of
the cell and eventually forms two separate polar Z rings; these developments require the SpollE protein. Only one polar site is used initiation
of septation at one site blocks the other site. [Science (2002) 298 19421946.]
During vegetative growth, SinR (encoded by sinR in the lower dashed box) represses expression of the spoII genes (dashed box, centre
right). During sporulation, Spo0AP represses abrB (lower dashed box) thus (indirectly) inhibiting expression of SinR and helping to promote
expression of the spoII genes; SinR is repressed at the proteinprotein level, i.e. inhibited by the SinI protein. Note that Spo0AP also directly
promotes the transcription of sinI. (Continued on page 273.)
272
stage 0
stage I
stage II ii
stage II iii
stage II i
stage III
exosporium
spore coat
cortex
cytoplasm
cytoplasmic core
membrane
stage IV
stages VVI
stage VII
273
endosporium
(See also ENDOTOXIC SHOCK.)
endotrophic mycorrhiza See MYCORRHIZA.
Endotrypanum A genus of protozoa (family TRYPANOSOMATIDAE)
parasitic in the erythrocytes of sloths (in Central and South
America) and in sandflies (Lutzomyia spp) which transmit
the protozoon to sloths. One species (E. schaudinni ) forms
intraerythrocytic epimastigotes, the other (E. monterogei ) forms
intraerythrocytic trypomastigotes; in culture both species form
promastigotes.
endotunica See BITUNICATE ASCUS.
endoxylanase See XYLANASES.
endozoite (tachyzoite) In certain coccidia: a stage within host
tissues (see e.g. TOXOPLASMOSIS).
energy charge (EC) See ADENYLATE ENERGY CHARGE.
energy-transducing membrane Any biological membrane which
contains components that are involved in the conversion of
one form of energy (e.g. light, ATP) to another (metabolically
usable) form of energy. Such membranes are involved e.g. in
RESPIRATION and PHOTOSYNTHESIS; they include the bacterial CYTOPLASMIC MEMBRANE (and the CHLOROSOME and CHROMATOPHORE
membranes), the inner membrane of the MITOCHONDRION, the
THYLAKOID membranes of cyanobacteria and CHLOROPLASTS, and
the PURPLE MEMBRANE in certain halobacteria. (In cyanobacteria,
respiratory electron transport occurs in the cytoplasmic membrane and, in at least some species, may occur also (in addition
to photosynthetic electron transport) in the thylakoids [Book
ref. 75, pp. 199218].) (See also CHEMIOSMOSIS.)
enFeLV viruses See FELINE LEUKAEMIA VIRUS.
enhancement effect (Emerson enhancement effect) In algae and
green plants illuminated with light of wavelength above ca.
680 nm: an increase in PHOTOSYNTHESIS which occurs when the
illumination is augmented with an additional beam of light of
shorter wavelength. (cf. RED DROP.)
enhancer A cis-acting DNA sequence, present in the genomes
of higher eukaryotes and of various animal viruses, which
can greatly increase transcription; an enhancer can generally
function in either orientation and at various distances (upstream
or downstream) from a given promoter. (cf. UAS.) The enhancer
of e.g. simian virus 40 (SV40) can function in a wide variety
of animal cells, but enhancers of certain other viruses and of
cellular genes show more or less strict specificity for particular
cell or tissue types. Enhancer function requires the participation
of trans-acting protein factors; for example, the SV40 enhancer
apparently consists of multiple elements, each of which is
recognized and bound by specific transcription factors [Book
ref. 189, pp. 1926]. Interactions between protein factors bound
to enhancers and to other genetic elements (e.g. PROMOTER) may
be important; in yeast, DNA looping between enhancer and
promoter suggests that apposition of these elements is involved
in enhancer action [NAR (2005) 33 37433750].
enhancer (translational) See DOWNSTREAM BOX.
enhancer-dependent sigma factor (s54 ) See SIGMA FACTOR.
enniatins Cyclic DEPSIPEPTIDE ANTIBIOTICS, obtained e.g. from
Fusarium spp, which behave as IONOPHORES (for monovalent
cations) and which are active against certain Gram-positive bacteria, e.g. Mycobacterium tuberculosis. The enniatin molecule
includes three residues of D-a-hydroxyisovaleric acid, each
occurring between two residues of N-methyl-L-isoleucine (enniatin A), N-methyl-L-valine (enniatin B ), N-methylleucine (enniatin C ), or N-methylphenylalanine (beauvericin, produced by
Beauveria bassiana); the residues are linked by alternating peptide and ester bonds.
enokitake (winter mushroom) Flammulina velutipes, a mushroom cultivated for food e.g. in Japan. Enokitake is grown on
Enteridium
sawdust supplemented with rice bran; the mycelium is grown
at 2025 C, and fruiting is induced by lowering the temperature to 1012 C. The cultivated fruiting bodies differ from
those which develop in nature, the mushroom being whitish or
cream-coloured with a long slender stipe. [Mycol. (1983) 75
351360.]
enoxacin See QUINOLONE ANTIBIOTICS.
enoyl-acyl carrier protein reductase (ENR) See DIAZABORINES
and TRICLOSAN.
enriched medium Any (liquid or solid) basal MEDIUM which has
been supplemented (enriched) with serum or blood etc or with
any of a range of nutrients or growth factors in order to enable
it to support or enhance the growth of particular type(s) of
organism. Examples: BLOOD AGAR, serum sugars (see PEPTONEWATER SUGARS). (cf. ENRICHMENT MEDIUM.)
enrichment Any process which increases the proportion of a
given microorganism in a mixed population. For example, faeces
from a typhoid case can be cultured in an enrichment medium
(e.g. SELENITE BROTH) which suppresses growth of the normal
faecal flora while permitting growth of the pathogen, Salmonella
typhi ; S. typhi is therefore enriched so that its detection is
facilitated. (See also DEFECTIVE INTERFERING PARTICLE.)
enrichment medium Any medium used for ENRICHMENT; it may
contain substance(s) which encourage growth of the required
organism and/or inhibit the growth of other type(s) of organism. (See e.g. SELENITE BROTH and TETRATHIONATE BROTH; cf.
ENRICHED MEDIUM.)
Ensifer A genus of Gram-negative, aerobic, chemoorganotrophic
and facultatively predatory, soil-inhabiting BUDDING BACTERIA;
cells: rod-shaped (ca. 0.71.1 1.01.9 m), motile by means
of a subterminal tuft of 35 flagella. The cells of E. adhaerens
(the type species) attach, end on, to a suitable prey bacterium
(e.g. Micrococcus luteus), forming a palisade arrangement; under
certain conditions the prey cell may be lysed. [IJSB (1982) 32
339345.]
ensiform Sword-like; narrow and pointed.
ensilage (1) The process of making SILAGE. (2) The silage itself.
Ent plasmid Any plasmid carrying genes for the ST and/or LT
enterotoxins of ETEC (q.v.).
entA gene (Staphylococcus aureus) See ENTEROTOXIN.
entAentG genes (in Escherichia coli ) See SIDEROPHORES.
Entamoeba A genus of protozoa (order AMOEBIDA) characterized
by the presence of beaded chromatin on the inner surface of
the nuclear membrane. Most species (not E. gingivalis) form
cysts which may contain CHROMATOID BODIES and glycogencontaining vacuoles. All species except E. moshkovskii occur
as parasites/commensals in the alimentary tract in animals.
E. coli. A non-pathogen found in human faeces. Trophozoites
are ca. 1050 m diam., contain numerous vacuoles, and slowly
form blunt, granular pseudopodia; the single karyosome is
located eccentrically, and the peripheral chromatin is coarsely
and irregularly beaded. Mature cysts contain 8 nuclei.
E. gingivalis. A non-pathogenic, non-cyst-forming species
found in the mouth in man and other animals. Trophozoites: ca. 535 m diam., morphologically similar to those of
E. histolytica.
E. hartmanni. A non-pathogenic species found in human faeces. It resembles E. histolytica, but both trophozoites (510 m
diam.) and cysts (<10 m diam.) are smaller.
E. histolytica. A parasite and potential pathogen in the human
intestine; it can cause amoebic DYSENTERY. Non-invasive trophozoites living in the gut lumen are ca. 20 m in diam.; invasive
forms which penetrate and develop in the gut mucosa are usually 2050 m diam. The cells contain few vacuoles, but may
contain ingested red blood cells (an almost pathognomonic feature); finger-shaped, hyaline pseudopodia are produced rapidly.
The (single) nucleus contains a small central karyosome, and the
peripheral chromatin is finely and regularly beaded. In the gut
lumen, some trophozoites expel their food particles and shrink
to become rounded, non-motile precysts; a precyst secretes a
resistant wall and becomes a spherical CYST (usually >10 m
and <20 m diam.). A cyst initially contains a single nucleus,
but two nuclear divisions result in four nuclei in the mature
cyst; each nucleus contains a central karyosome. Young cysts
may contain round-ended chromatoid bodies in the cytoplasm.
Trophozoites, precysts and cysts may all be found in the faeces
of the host, but only the cysts are infective for another host.
Cysts are resistant to various environmental conditions and
to normal chlorination levels in water supplies but are sensitive to temperatures >40 C and < 5 C and to desiccation.
Cysts may be stained with iodine (cytoplasm yellow, glycogen vacuoles reddish-brown); trophozoites stain well with e.g.
ironhaematoxylin after fixation in PVA (cytoplasm grey or pale
violet, nuclear structures black). E. histolytica may be cultured
anaerobically on media containing e.g. inspissated horse serum,
rice starch, or egg albumen, together with bacteria or flagellate
protozoa; it has also been cultured in sterile media. Strains have
been classified on the basis of growth characteristics (classical strains grow best at 37 C, while atypical, less pathogenic
Laredo-type strains grow well at 37 C and at 25 C), or by the
presence or absence of the enzyme phosphoglucomutase (present
in organisms from patients with clinical amoebiasis, but not in
those from asymptomatic carriers). (See also PYROPHOSPHATE.)
E. moshkovskii. A non-pathogen found in sewage; it resembles
E. histolytica morphologically, but apparently occurs only in the
free-living state.
E. paulista. A hyperparasite found in the cytoplasm of
Opalina ranarum in frogs.
Other species include e.g. E. bovis (from cattle), E. invadens
(pathogenic in reptiles), E. muris (from rats and mice), and
E. polecki (from pigs).
[Biochemistry and functional morphology of Entamoeba: JP
(1985) 32 221240.]
enteric Of or relating to the intestine (particularly the small
intestine). Enteric bacteria may refer to any or all bacteria
normally found in the (small or large) intestine, or may refer
specifically to members of the ENTEROBACTERIACEAE.
enteric adenoviruses See MASTADENOVIRUS.
enteric fever Any typhoid-like human salmonellosis caused
e.g. by Salmonella paratyphi (cf. PARATYPHOID FEVER), S. typhimurium etc. as distinct from Salmonella FOOD POISONING.
Some authors include TYPHOID FEVER among the enteric fevers.
enteric redmouth (red vent disease) A disease of rainbow trout
(Salmo gairdneri ) caused by Yersinia ruckeri. Symptoms include
e.g. haemorrhagic lesions in and around the mouth and vent. (cf.
RED MOUTH.)
enteric septicaemia (of fish) A disease of the channel catfish
(Ictalurus punctatus) caused by Edwardsiella ictaluri ; the disease has become an important problem in the intensive cultivation of catfish. Naturally infected fish often have a characteristic
erosive lesion on the head (hole-in-the-head); chronic cases
may involve enteritis, hepatitis, meningoencephalitis, etc. Primary infection can apparently occur via the gut or via the nares.
[Pathogenesis: CJFAS (1986) 43 3642.] (See also FISH DISEASES.)
Enteridium See MYXOMYCETES.
275
enteritis
Enterobacteriaceae A family of Gram-negative, asporogenous,
facultatively anaerobic bacteria. Cells: rod-shaped, typically
ca. 0.31.0 16 m (cf. OBESUMBACTERIUM), motile (peritrichously flagellate cf. TATUMELLA) or non-motile. Metabolism
is chemoorganotrophic and may be respiratory or fermentative,
depending e.g. on conditions. Most species can reduce nitrate
to nitrite. All species are oxidase ve and (except for Shigella
dysenteriae serotype 1 and Xenorhabdus nematophilus) catalase +ve. Reproduction occurs by binary fission. Type genus:
Escherichia.
Enterobacteria occur e.g. as parasites, pathogens or commensals in man and/or animals, as saprotrophs or pathogens in plants
(see ERWINIA), or as saprotrophs (or faecal contaminants) in soil
and water. Many are important opportunist causes of nosocomial
infections.
Enterobacteria typically grow readily on a range of basal
media (e.g. NUTRIENT AGAR). Media selective for enterobacteria
commonly contain a sugar (often lactose), bile salts (as selective
agents), and a pH indicator (see e.g. MACCONKEYS AGAR).
Genera and species are traditionally differentiated on the
basis of biochemical tests e.g. the IMVIC TESTS, the ability to
produce certain enzymes (e.g. UREASE, ARGININE DIHYDROLASE),
to utilize particular sugars (mono- and disaccharides, polyols
etc), to decarboxylate or deaminate certain amino acids (see
e.g. DECARBOXYLASE TEST), to produce HYDROGEN SULPHIDE from
thiosulphate (see e.g. TSI AGAR), etc. [Identification tests: Book
ref. 184.] Reactions to such tests may be affected e.g. by
mutation or by the presence of a metabolic PLASMID, and in
some cases are strongly dependent on the reaction conditions
(see e.g. YERSINIA). DNA HOMOLOGY (DNA relatedness) studies
have been widely used to indicate degrees of relatedness between
strains, species and genera. However, the genera Escherichia
and Shigella, for example, continue to be recognized even
though they have been shown to be sufficiently closely related
genetically to be regarded as a single genus (or even as a single
species). [Book ref. 46, pp. 11081112.]
Many enterobacteria can be serotyped (see TYPING) on the
basis of O ANTIGENS, H ANTIGENS, K ANTIGENS and/or VI ANTIGENS; cross-reactions between members from different genera
are quite common (see e.g. CITROBACTER). All enterobacteria
(except Erwinia chrysanthemi ) possess the ENTEROBACTERIAL
COMMON ANTIGEN. Colicin, bacteriophage and antibiotic TYPING
may be used for particular genera. [Serology/serotyping in enterobacteria: Book ref. 68.]
Genera: CEDECEA; CITROBACTER; EDWARDSIELLA; ENTEROBACTER; ERWINIA; ESCHERICHIA; EWINGELLA; HAFNIA; KLEBSIELLA;
KLUYVERA; KOSERELLA; LEMINORELLA; MOELLERELLA; MORGANELLA; OBESUMBACTERIUM; PROTEUS; PROVIDENCIA; RAHNELLA;
SALMONELLA; SERRATIA; SHIGELLA; TATUMELLA; XENORHABDUS;
YERSINIA. (See also SODALIS.)
enterobacterial common antigen (ECA; Kunin antigen) A heteropolysaccharide antigen found in the outer membrane in all
wild-type strains of the Enterobacteriaceae (excluding Erwinia
chrysanthemi ) and e.g. in strains of PLESIOMONAS. It consists of
alternating residues of (1 4)-linked N-acetyl-D-glucosamine
and N-acetyl-D-mannosaminuronic acid which may be esterified
with small amounts of e.g. palmitic and acetic acids. ECA may
be linked to phospholipid (when it is poorly immunogenic), or it
may be bound e.g. to the core region of LPS (when it is highly
immunogenic); it is readily accessible to homologous antibodies
in non-capsulated rough strains, but may be inaccessible e.g. in
smooth, capsulated strains [JGM (1982) 128 15771583].
enterobacterial repetitive intergenic consensus sequence See
ERIC SEQUENCE.
enteritis Inflammation of the lining of any part of the intestine particularly the small intestine; it may result from the
same causes as GASTROENTERITIS. (cf. COLITIS.)
enteritis necroticans (necrotizing enteritis; pig bel; Darmbrand)
A rare, severe (often fatal), haemorrhagic enteric disease caused
by ingestion of food (commonly pig meat) contaminated with
Clostridium perfringens type C. (cf. FOOD POISONING.) The organisms adhere to the intestinal mucosa and produce the necrotizing
b-toxin, causing necrosis of the mucosa. Diet influences disease development: the b-toxin is normally readily inactivated
by digestive proteases; however, high-carbohydrate, low-protein
diets reduce the secretion of proteases, and e.g. sweet potatoes
contain a trypsin inhibitor which further lowers proteolytic activity factors which allow the b-toxin to persist.
enteroadherent E. coli Diarrhoeagenic strains of Escherichia
coli characterized by their ability to adhere to (mammalian)
HEp-2 cells; strains can be differentiated on the basis of their
patterns of adherence: diffusely adherent E. coli (DAEC)
adheres primarily as isolated, individual cells in a diffuse
manner, while enteroaggregative E. coli (EAggEC: see EAGGEC)
forms a pattern of scattered aggregates in which most of the
cells are obviously grouped with other cells. (EPEC adheres
to HEp-2 in a localized manner, forming microcolonies.) The
category enteroadherent has been discontinued: strains of HEp2-adherent E. coli (excluding EPEC) are now divided into the
two main groups EAggEC and DAEC (each of which, though
still heterogeneous, is associated with distinct virulence factors
and epidemiology) [RMM (1995) 6 196206].
(See also EAEC.)
enteroaggregative E. coli See EAGGEC.
Enterobacter A genus of Gram-negative bacteria of the ENTEROBACTERIACEAE (q.v.). Cells: ca. 0.61.0 1.23.0 m, motile
(generally 46 peritrichous flagella). Most strains possess fimbrial haemagglutinins [JGM (1983) 129 21752180]. Typical
reactions: indole ve; MR ve; VP +ve; citrate +ve; H2 S ve;
acid and gas from glucose at 37 C (no gas at 44.5 C); lactose
+ve. Optimum growth temperature: ca. 30 C. GC%: 5260.
Type species: E. cloacae.
Enterobacter spp occur e.g. in the intestines of man and
animals, in soil, water and sewage, in foods (e.g. dairy products),
on plants etc. Most species can be opportunist pathogens, causing
nosocomial infections (e.g. meningitis, pneumonia, septicaemia,
UTI).
E. aerogenes. Lysine and ornithine decarboxylases +ve; arginine dihydrolase ve; D-sorbitol +ve; non-pigmented. (It has
been proposed that E. aerogenes be transferred to the genus
Klebsiella as K. mobilis [see Book ref. 22, p. 463, 466 and
469].) (cf. AEROBACTER.)
E. agglomerans. A heterogeneous species comprising organisms alternatively included in Erwinia herbicola (see ERWINIA).
Lysine and ornithine decarboxylases ve; arginine dihydrolase
ve; lactose ve. Some strains are yellow-pigmented.
E. cloacae. Lysine decarboxylase ve; ornithine decarboxylase +ve; arginine dihydrolase +ve; D-sorbitol +ve; DNase ve
at 25 C. Non-pigmented. Naturally resistant to ampicillin.
E. sakazakii includes yellow-pigmented strains previously
included in E. cloacae. D-Sorbitol ve; DNase delayed +ve at
25 C.
Other species: E. amnigenus, E. gergoviae, E. intermedium.
(E. hafniae and E. alvei : see HAFNIA; E. liquefaciens: see SERRATIA.)
[Book refs. 46, pp. 11731180; and 22, pp. 465469.]
enterobacteria Bacteria of the ENTEROBACTERIACEAE.
276
Enterovirus
enterobactin See SIDEROPHORES.
enteroblastic proliferation (mycol.) See CONIDIUM.
enterochelin See SIDEROPHORES.
enterochromaffin cells Cells in the mammalian gut epithelium
which secrete certain hormones e.g. SEROTONIN (a stimulator
of intestinal secretion).
enterocin P A broad-spectrum BACTERIOCIN produced by Enterococcus faecium strain P13 and secreted by a sec-dependent pathway; it inhibits strains of e.g. Listeria monocytogenes, Staphylococcus aureus, Clostridium perfringens and C. botulinum. [Biochemical and genetic characterization of enterocin P: AEM
(1997) 63 43214330.]
enterococci (1) Members of the genus ENTEROCOCCUS. (2) A term
which has been used very loosely to refer to some or all of the
organisms referable to the genus ENTEROCOCCUS.
Enterococcus A genus of Gram-positive, asporogenous, chemoorganotrophic, facultatively anaerobic, coccoid bacteria; the
genus was originally proposed to accomodate organisms previously classified as Streptococcus faecalis and Streptococcus
faecium [proposal to transfer S. faecalis and S. faecium to the
genus Enterococcus as E. faecalis and E. faecium respectively:
IJSB (1984) 34 3134]. [Proposal to transfer other streptococci
to this genus: S. avium (as Enterococcus avium), S. casseliflavus
(E. casseliflavus), S. durans (E. durans), S. faecalis subsp malodoratus (E. malodoratus) and S. gallinarum (E. gallinarum):
IJSB (1984) 34 220223.]
Members of the genus occur in the animal and human
intestine; they can usually grow at 10 C and 45 C, and can
grow in 6.5% sodium chloride and at pH 9.6. Metabolism:
typically fermentative, but at least some strains can carry
out respiratory metabolism when provided with haemin under
aerobic conditions. (See also PYR.) GC% 3745. Type species:
E. faecalis.
E. faecalis. Organisms formerly classified as Streptococcus
faecalis (Lancefield group D). Cells: ovoid, occurring singly or
in pairs or short chains; motile strains are rare. Non-haemolytic
or, rarely, b-haemolytic. E. faecalis can survive 60 C/30 min.
Various sugars are fermented (e.g. D-tagatose, but not e.g. D- or
L-arabinose), and acid is formed from glycerol both aerobically
and anaerobically. Energy can be obtained from pyruvate, citrate
and malate. Growth can occur in the presence of 0.02% sodium
AZIDE, 0.04% tellurite, or 0.01% TETRAZOLIUM. Some strains
form a PSEUDOCATALASE.
Some strains of E. faecalis can transmit/receive plasmids that
confer resistance to antibiotic(s) (see CONJUGATION). A current
problem is the acquisition of (plasmid-borne) resistance to VANCOMYCIN; the appearance of vancomycin-resistant enterococci
(VRE) is important because enterococci are frequent causal
agents of nosocomial bacteraemia. It has been estimated that
15% of enterococci are resistant to vancomycin [EID (1998)
4 239249]. Vancomycin resistance may be conferred by one
or more plasmid-borne van genes; vanA and vanB both confer resistance to vancomycin, while vanA also confers resistance
to teichoplanin. (These two genes have been reported in both
E. faecalis and E. faecium.) Multiplex PCR has been used for
rapidly detecting vanA and vanB in presumptive colonies of
VRE [JCM (1999) 37 20902092].
[Vancomycin-resistant E. faecium with a VanB phenotype in
a Warsaw hospital: JCM (2001) 39 17811787.]
E. faecium. Organisms formerly classified as Streptococcus faecium (Lancefield group D). The organisms resemble
E. faecalis in morphology and general characteristics, including
resistance to heat, high pH and salinity; some strains are ahaemolytic. Acid is formed from arabinose but not from tagatose.
EntnerDoudoroff pathway
taken into the cell by specific transport systems and then phosphorylated to form 6-phosphogluconate (which can then be
metabolized via the ED pathway and/or the HMP pathway).
[ED pathway (history, physiology, molecular biology): FEMS
Reviews (1992) 103 128. ED pathway in E. coli: JB (1998)
180 34953502.]
Entodiniomorphida An order of protozoa (subclass VESTIBULIFERIA) in which the cells are naked except for tufts or bands of
oral and (often) somatic syncilia. STOMATOGENESIS is apparently
apokinetal. In some species the pellicle is drawn out into terminal spikes or spines. The organisms occur e.g. in the alimentary
canal in herbivorous mammals. Genera: e.g. DIPLODINIUM, ENTODINIUM, Epidinium, Metadinium.
Entodinium
A genus of ciliates (order ENTODINIOMORPHIDA)
related to DIPLODINIUM. Typically, the anterior pole of the cell is
flattened and bears a conspicuous tuft of cilia; there is no DZM,
and the posterior end of the cell may or may not be drawn out
into spines.
entomo- Prefix denoting insecte.g. entomopathology: the study
of INSECT DISEASES; entomopathogenic: pathogenic for insects.
entomogenous Growing in or on insects.
entomopathogenic Pathogenic for insects (see INSECT DISEASES).
Entomophaga See ENTOMOPHTHORALES.
Entomophthora A genus of fungi (order ENTOMOPHTHORALES)
which include saprotrophs and parasites of insects. The vegetative thallus is commonly an aseptate or septate mycelium with a
tendency to fragment; the conidia are forcibly discharged. AZYGOSPORES are formed by some species. [Key to Entomophthora
(sens. lat.): BBMS (1982) 16 113143; infection of houseflies
by E. muscae: TBMS (1983) 80 18; ultrastructural studies of
primary spore formation and discharge in Entomophthora: J.
Inv. Path. (1986) 48 318324.]
Entomophthorales An order of fungi (class ZYGOMYCETES)
which include a number of parasites of insects and mammals.
Asexually derived spores often called conidia are forcibly
discharged in members of the families Basidiobolaceae and
Entomophthoraceae. (Members of the ZOOPAGALES are sometimes included as a third family in this order.) Genera include
Basidiobolus (see also ZYGOMYCOSIS and EQUINE PHYCOMYCOSIS)
and (in the family Entomophthoraceae) Conidiobolus (see also
ZYGOMYCOSIS), Entomophaga, ENTOMOPHTHORA, ERYNIA, Gonimochaete (see NEMATOPHAGOUS FUNGI), and Zoophthora. (See
also LOBOA and HYPHAL BODY; cf. BLASTOCYSTIS.)
entomophthoromycosis See ZYGOMYCOSIS.
Entomopoxvirinae (entomopoxviruses, EPVs) A subfamily of
viruses, family POXVIRIDAE, which infect insects including
members of the Coleoptera (beetles etc), Diptera (flies etc), Lepidoptera (butterflies and moths), and Orthoptera (locusts, crickets,
grasshoppers etc). EPV virions are brick-shaped or ovoid, ca.
300450 170250 nm, with a characteristic mulberry-like
appearance in negatively stained preparations the globular surface units apparently being folds of the outer membrane. The
viruses multiply in the cytoplasm of (mainly) leucocytes and adipose cells of the host. Late in the replication cycle infected cells
may contain one or two types of inclusion body: spheroids (=
spherules, each consisting of mature virions occluded within a
matrix of protein, spheroidin) and spindles (virus-free, spindleshaped structures composed of a protein which is apparently
distinct from spheroidin). A new host is infected when it ingests
a spheroid and the virions are released in the alkaline contents of
the gut. EPVs apparently vary in their pathogenicity, but at least
some can cause diseases (spheroidoses) in their hosts; they are
currently little used for biological control of insect pests.
enzyme
Such viruses are taken up (intact) by the host cell by receptormediated endocytosis, and only when the contents of the
endosome become sufficiently acidic does fusion occur between
the viral envelope and the endosomal membrane resulting in
the release of the nucleocapsid into the cytoplasm. [Review of
endocytosis of enveloped viruses: Bioch. J. (1984) 218 110.]
In many enveloped viruses (e.g. influenzaviruses) the individual virions do not share a common structure or composition; for
example, the envelope glycoproteins in influenzaviruses do not
occur in a fixed number in all the virions. By contrast, a defined
structure is found in the virions of alphaviruses and flaviviruses
[see e.g. Cell (2001) 105 58].
In most cases a virus acquires its envelope (during virion
assembly) by a process of budding (cf. FLAVIVIRIDAE). The virusencoded envelope proteins each contain an anchor peptide (see
SIGNAL HYPOTHESIS) and become anchored in the appropriate cell
membrane (e.g. endoplasmic reticulum, plasmalemma, nuclear
membrane according to virus); these proteins then interact
with proteins in the preformed nucleocapsid, causing the associated region of membrane to wrap around the nucleocapsid. This
region of membrane eventually becomes detached from the host
membrane, completing the assembly process.
Enveloped virions are typically readily inactivated by lipiddisrupting reagents and procedures: e.g. organic solvents such
as ether and chloroform, detergents, heat, etc.
[Membranes in animal viruses: Book ref. 148, pp. 4567.]
(2) (bacteriol.) Syn. CELL ENVELOPE.
environmental clean-up See BIOREMEDIATION.
environmental pollution See e.g. BIOREMEDIATION, GREENHOUSE
EFFECT, SEWAGE TREATMENT, WATER SUPPLIES and XENOBIOTIC.
(See also AEROSOL and AIR.)
enviroxime (2-amino-1-(isopropylsulphonyl)-6-benzimidazolylphenyl ketone oxide) An ANTIVIRAL AGENT which specifically
inhibits rhinovirus replication in cell cultures; it does not appear
to be effective in preventing or treating human rhinovirus infections in vivo.
EnvZ See OSMOREGULATION.
enzootic Refers to an ENDEMIC animal disease.
enzootic abortion (enzootic ovine abortion) Abortion in sheep
caused by Chlamydia psittaci. Laboratory diagnosis may involve
e.g. detection by microscopy of elementary bodies in stained
placental smears, or culture of placental material [VR (1983)
113 413414]. (cf. INFECTIOUS ABORTION.)
enzootic bovine leukaemia Syn. BOVINE VIRAL LEUKOSIS.
enzootic ovine abortion See ENZOOTIC ABORTION.
enzootic pneumonia of calves See CALF PNEUMONIA.
enzyme A protein which acts as a highly efficient and specific
biological catalyst. (Certain RNA molecules are capable of
catalytic activity in the absence of protein, and these are
sometimes called enzymes (cf. RIBOZYME); the account below
refers specifically to protein catalysts.) An enzyme increases the
rate of a (thermodynamically feasible) reaction by decreasing
the activation energy; it cannot alter the equilibrium constant
of a reaction. Many enzymes require non-protein COENZYMES,
PROSTHETIC GROUPS, or metal ions/atoms for activity. (See also
ZYMOGEN.)
Most enzymes have trivial names which usually indicate
the nature of the substrate(s) and/or the reaction catalysed
(e.g. urease splits urea, alcohol dehydrogenase dehydrogenates
alcohol). However, a systematic scheme for the classification
and precise nomenclature of enzymes has been established by
the IUB Commission on Enzymes. The classification involves
the division of all known enzymes into six general classes
epidemiology
a stroma, the asci each containing eight filiform ascospores
which often fragment in the ascus. E. typhina causes CHOKE.
(See also FESCUE FOOT and ENDOPHYTE.)
epicone See DINOFLAGELLATES.
epidemic In a human population within a given geographical
region: an outbreak of an infectious disease in which, for a
limited period of time, a high proportion of individuals in
the population exhibits overt symptoms of the disease (cf.
ENDEMIC); epidemics are characterized by a sudden onset. (An
analogous outbreak of disease among animals or plants is called
an epizootic or epiphytotic, respectively.) (See also PANDEMIC
and EPIDEMIOLOGY.)
Currently, the term epidemic is often used in a broader sense
to include the occurrence of any disease either infectious or
non-infectious whose incidence in a given population clearly
exceeds that common in other populations.
epidemic encephalitis Syn. VON ECONOMOS ENCEPHALITIS.
epidemic haemorrhagic fever Syn. KOREAN HAEMORRHAGIC
FEVER.
epidemic hepatitis Syn. HEPATITIS A.
epidemic keratoconjunctivitis (shipyard eye) A highly infectious KERATOCONJUNCTIVITIS caused by an adenovirus (commonly
Ad8: see MASTADENOVIRUS). Infection appears to require direct
inoculation of the eye and is typically acquired from inadequately disinfected ophthalmological instruments, contaminated
eye ointments etc. (The virus is resistant to organic solvents
such as alcohol.) Conjunctivitis with oedema, pain, photophobia and a watery discharge may be followed by erosion of the
cornea sometimes resulting in permanent visual impairment.
epidemic meningitis Meningococcal MENINGITIS.
epidemic myalgia Syn. BORNHOLM DISEASE.
epidemic spread (infectious spread) (of plasmids) An effect
which occurs when a population of conjugal donor cells (see
CONJUGATION sense 1b), carrying a plasmid that is repressed for
transfer, is mixed with a population of recipient cells. Initially,
a small proportion of the donor cells becoming spontaneously
DEREPRESSED for transfer donate their plasmids to recipient
cells (low frequency transfer ; LFT). In each of these recipient
cells, the newly acquired plasmid remains derepressed owing to
the absence of repressor molecule(s); such a cell, and/or progeny
derived from it, can transmit the plasmid to a fresh recipient. This
effect is cumulative, resulting in the rapid (epidemic) spread of
the plasmid throughout the population (high frequency transfer ;
HFT). Cells in the HFT state gradually (over several generations)
become repressed for transfer as the intracellular concentration
of repressor molecule(s) builds up.
epidemic tremor Syn. AVIAN ENCEPHALOMYELITIS.
epidemic vomiting disease See FOOD POISONING (i).
epidemiology The study of the interrelationships between a
given pathogen, the environment, and groups or populations
of the relevant hosts; the object is to investigate the factors
and mechanisms which govern the spread of disease within
a community or population. Three main factors are involved.
(a) The virulence of the pathogen. Since the observed virulence
of a pathogen is related to host susceptibility (a variable)
it is difficult to define virulence in absolute terms. (b) Herd
immunity. This may be regarded as the collective immunity
or resistance to a given disease exhibited by a community
or population (human or animal) in the setting of its own
environment. (Immunity in individual members of a population
may result from e.g. VACCINATION or recovery from the disease.)
An important feature of herd immunity is the ratio of immunes
(individuals resistant to the disease) to susceptibles (those
epidermin
is unknown; neither is it known why toxin-producing strains
produce localized lesions (impetigo) in some individuals and
extensive, spreading scalding lesions in others. [Book ref. 44,
pp. 599617.]
Epidermophyton See DERMATOPHYTES.
Epidinium A genus of ciliates related to DIPLODINIUM.
epifluorescence microscopy See MICROSCOPY (e).
epigean Occurring on the surface of the ground (cf. HYPOGEAN).
epiglottitis Inflammation of the epiglottis. Acute epiglottitis is
a life-threatening condition caused primarily by Haemophilus
influenzae; it occurs mainly in small children. Fever and sore
throat are followed rapidly by inspiratory stridor and dysphagia;
the epiglottis becomes oedematous and cherry-red, and may
cause complete respiratory obstruction.
epilimnion The surface layer of a lake which, due to thermal
effects and wind, is well-mixed and aerobic and approximately
uniform in temperature. (cf. METALIMNION.)
epilithic Growing on the surface of rock or stone etc. (cf.
SAXICOLOUS.)
epilithon The community of sessile organisms which grow on
the surfaces of underwater stones. [Composition of epilithon:
Oikos (1984) 42 1022.]
epimastigote A form assumed by the cells of species of Blastocrithidia, Endotrypanum and Trypanosoma during at least
certain stages of their life cycles: see TRYPANOSOMATIDAE.
epimerite In cephaline gregarines: a differentiated region of
the PROTOMERITE, delineated by a septum, by means of which
the developing parasite remains attached to the host cell (cf.
MUCRON).
epimicroscopy See MICROSCOPY (g).
epinasty (plant pathol.) The downward curvature of a plant
structure (particularly a leaf petiole) due to the faster growth
of the dorsal side of the structure relative to the ventral side.
Epinasty can be induced e.g. by ETHYLENE, and is an early
symptom in certain plant diseases.
epinephrine Syn. ADRENALIN (q.v.).
epineuston See NEUSTON.
epipelic Growing on mud.
epiphloeodal (epiphloedal) Growing on the surface of bark (cf.
CORTICOLOUS).
epiphragm See CYATHUS.
epiphyte A plant or plant-like organism (e.g. a lichen) which
grows upon another plant but does not derive nutrients from
it i.e., an epiphyte is non-parasitic. (cf. ENDOPHYTE.)
epiphytotic See EPIDEMIC.
epiplan objective A FLAT-FIELD OBJECTIVE LENS used for brightfield epimicroscopy (see MICROSCOPY (g)).
epiplasm (1) (protozool.) See PELLICLE. (2) (mycol.) That cytoplasm in an ASCUS which is not incorporated into ascospores.
epipodophyllotoxins See PODOPHYLLOTOXIN.
epipolythiapiperazinediones A group of fungal ANTIBIOTICS.
Some (e.g. aranotin, GLIOTOXIN, hyalodendrins, sirodesmins)
inhibit the replication of certain RNA viruses apparently by
binding to and inhibiting viral RNA-dependent RNA polymerase; however, they are too toxic for therapeutic use.
episome (1) A PLASMID which can exist either in an autonomous
(extrachromosomal) state or integrated in the host cells chromosome.
(2) Syn. PLASMID.
episporium See EXOSPORIUM (sense 2).
epistasis The dominance of one (epistatic) allele over a nonallelic (hypostatic) allele. (cf. DOMINANCE.)
Epistylis See PERITRICHIA.
EpsteinBarr virus
within the nucleus. EBNA-1 also appears to be required for
replication of the plasmid form of EBV. (See also ZEBRA.)
The ebna-1 gene is only one of nine or ten viral genes (out of
80) which may be expressed during viral latency. The ebna-2
gene is reported to be necessary for transactivation of lmp-1 and
lmp-2 whose products (the latency membrane proteins 1 and 2)
are incorporated into the B cell membrane.
The products of ebna-2, ebna-3A and ebna-3C may also be
expressed at the cell surface.
In addition to proteins, latent EBV gives rise to two small
polyadenylated RNA molecules called EBV-encoded RNAs
(EBER-1 and EBER-2); these molecules are expressed at high
levels, but their function is unknown. The EBERs have been
used as targets for detection of EBV.
Certain genes in latent EBV are also involved in the transactivation of some of the B cell genes; these B cell genes
encode e.g. ICAM-1 (see CD54), LFA-1 (see INTEGRINS) and LFA3 (see IMMUNOGLOBULIN SUPERFAMILY). CD23, a B-cell-encoded
activation-related marker, is also produced; this molecule is
reported to act as an autocrine B-cell growth factor when shed
from the cell surface.
In vivo, proliferating B cells (with cell-surface molecules
of EBNA-2, EBNA-3A, EBNA-3C and LMP-1) are normally
targeted by a subset of EBV-specific cytotoxic T cells; moreover,
these virus-infected immortalized B cells are targets for NK
(natural killer) cells, and are also susceptible to interferons. Thus,
the number of proliferating B cells is normally controlled in
immunocompetent individuals.
Cells containing latent EBV do not necessarily express all of
the proteins referred to above; in some cases, however, all of
these proteins (and others) may be expressed. In fact, several
different types of EBV latency have been distinguished. In
type I latency only EBNA-1 is produced. Cells which express
only EBNA-1 are found e.g. in some gastric carcinomas; as
these cells lack the targets for EBV-specific cytotoxic T cells
(see above) they escape this form of immune control. In
type II latency the cell expresses EBNA-1 and LMPs 1 and
2; this pattern is found e.g. in some T-cell lymphomas and in
nasopharyngeal carcinoma. In type III latency the cell expresses
the full complement of these proteins; this pattern is found e.g.
in B cells from the acute phase of infectious mononucleosis.
(EBERs appear to be expressed in all forms of latency.)
EBV-associated diseases include: BURKITTS LYMPHOMA; HAIRY
LEUKOPLAKIA; INFECTIOUS MONONUCLEOSIS; NASOPHARYNGEAL
CARCINOMA; XLP SYNDROME, gastric carcinoma and diffuse
polyclonal B-cell lymphomas. In both Burkitts lymphoma and
nasopharyngeal carcinoma, pathogenesis seems to depend on
proliferation of host cells latently infected with EBV, whereas
in hairy leukoplakia the main pathogenic mechanism appears
to involve viral replication; in infectious mononucleosis, the
immune response of the host appears to be a major factor in
pathogenesis.
Diagnosis of EBV-associated diseases involves laboratory
tests (see e.g. INFECTIOUS MONONUCLEOSIS) and clinical observation. Levels of positivity of anti-EBV antibodies have been
well documented, so that serology may help to distinguish e.g.
between a primary (initial) infection (or a previous infection)
and reactivation in the latter case higher levels of antibodies
are formed against viral capsid antigen (VCA), early antigen
(EA) and EBNA. The EBERs may be detected e.g. by in situ
hybridization or by RNA-amplification techniques.
Treatments for various EBV-associated diseases include
antivirals (such as ACYCLOVIR), immunosuppressants (e.g.
Epulopiscium fishelsoni
cyclophosphamide), anti-B cell monoclonal antibodies and
inferon-gamma (IFN-g).
[Haematological associations of EBV: BCH (2000) 13 199
214.]
Epulopiscium fishelsoni See BACTERIA.
EPV Entomopoxvirus: see ENTOMOPOXVIRINAE.
equal density centrifugation See CENTRIFUGATION.
equid (alpha) herpesvirus 1 See ALPHAHERPESVIRINAE.
equid herpesvirus 3 Syn. EQUINE COITAL EXANTHEMA virus.
equilibrium density gradient centrifugation See CENTRIFUGATION.
equilibrium zonal centrifugation See CENTRIFUGATION.
equine abortion virus See ALPHAHERPESVIRINAE.
equine arteritis virus See ARTERIVIRUS.
equine blastomycosis Syn. EPIZOOTIC LYMPHANGITIS.
equine coital exanthema An acute, usually mild, usually venereally transmitted HORSE DISEASE caused by equid herpesvirus
3 (see ALPHAHERPESVIRINAE). Typically, vesicular or papular
lesions develop on the external genitalia (sometimes also on the
conjunctivae, lips or nasal mucosa); the lesions progress rapidly
to pustules (which may ulcerate), and generally heal in ca. 2
weeks.
equine diseases See HORSE DISEASES.
equine encephalosis subgroup See ORBIVIRUS.
equine herpesvirus 2 See GAMMAHERPESVIRINAE.
equine histoplasmosis Syn. EPIZOOTIC LYMPHANGITIS.
equine infectious anaemia Syn. SWAMP FEVER.
equine monocytic ehrlichiosis Syn. POTOMAC HORSE FEVER.
equine phycomycosis (hyphomycosis destruens; swamp cancer;
bursattee; Florida horse leech) A tropical and subtropical
HORSE DISEASE characterized by ulcerating, spreading, granulomatous lesions on the skin and mucous membranes; the
lesions contain masses of yellow-grey necrotic tissue (grains,
leeches) which may calcify. The causal agent is Hyphomyces
destruens, a Pythium sp. In Australia, outbreaks are associated with grazing in areas of permanent standing water [TBMS
(1983) 80 1318]. Clinically similar conditions are caused e.g.
by Basidiobolus haptosporus and by certain helminthic parasites.
(See also ZYGOMYCOSIS.)
equine protozoal myeloencephalitis (equine protozoal myelitis)
A HORSE DISEASE which affects young and old horses of both
sexes; it occurs in certain areas of the USA. The symptoms
are those typical of CNS involvement; they include stumbling
and falling, sometimes with partial paralysis of the face and/or
tongue, muscle atrophy, and lameness. The causal agent is
believed to be a member of the coccidia (suborder EIMERIORINA)
[IJP (1987) 17 615620].
equine rhinoviruses See PICORNAVIRIDAE.
equivalence (serol.) Syn. OPTIMAL PROPORTIONS.
ER ENDOPLASMIC RETICULUM.
Era protein See CELL CYCLE (b).
eradicant (plant pathol.) Any chemical agent which eliminates
particular pathogen(s) from diseased plants treated with that
agent. (cf. PROTECTANT.)
erb
An ONCOGENE originally identified as the transforming
determinant in avian erythroblastosis virus (AEV: see AVIAN
ACUTE LEUKAEMIA VIRUSES). In AEV, v-erb consists of two
contiguous genes, v-erb-A and v-erb-B; the cellular homologues
(c-erb-A and c-erb-B) are not linked in the chicken genome.
The cellular homologue of v-erb-A (c-erb-A) encodes the
thyroid hormone receptor. This protein lacks tyrosine kinase
activity and is apparently not tumorigenic on its own.
The cellular homologue of v-erb-B (c-erb-B) encodes a
membrane protein that functions as the epidermal growth factor
Erysipelothrix
E. chrysanthemi. Pectinolytic. Causes vascular wilts in a wide
range of plants. Some strains produce a blue bipyridyl pigment,
indigoidine, on YGC agar.
E. herbicola. Common as saprotrophs on the surfaces of
land plants; some strains can fix nitrogen. May act as secondary invaders in plant lesions. (See also HERBICOLIN A.)
Some strains can cause GALL formation. Certain strains are
opportunist parasites or pathogens in man and animals; such
strains are regarded by clinical microbiologists as Enterobacter
agglomerans. [Attempted classification of strains of the HerbicolaAgglomerans group: IJSB (1984) 34 4555.]
E. nigrifluens. Causes bark necrosis of Persian walnut (Juglans
regia).
E. rhapontici. Causes e.g. crown rot of rhubarb (Rheum
rhaponticum) and pink grain of wheat; it can also grow
saprotrophically in plant lesions. A pink diffusible pigment is
formed on sucrosepeptone agar.
E. rubrifaciens. Pectinolytic. Causes phloem necrosis (bark
canker) of Persian walnut (Juglans regia). A pink pigment is
produced on YGC agar.
E. salicis. Pectinolytic. Causes WATERMARK DISEASE in willows
(Salix spp). Produces yellow pigment on autoclaved potato
tissue.
E. stewartii. Non-motile. Causes vascular wilt of e.g. maize
(Zea mays); overwinters primarily in the flea beetle Chaetocnema pulicaria.
E. tracheiphila. Causes vascular wilt in Cucurbita spp; overwinters in cucumber beetles (Diabrotica spp).
E. uredovora. A parasite of the uredia and uredospores of
Puccinia graminis. Produces yellow pigment on nutrient agar.
Other recognized species: E. ananas (causes pineapple rot),
E. cypripedii, E. mallotivora, E. quercina.
[Taxonomy: Book ref. 22, pp. 469476. Habitats, culture etc:
Book ref. 46, pp. 12601271.]
See also COFFEE; PECTIC ENZYMES.
Erynia
A genus of fungi (order ENTOMOPHTHORALES) which
include parasites of insects; E. neophidis is a pathogen of aphids.
[Persistence of infectious spores of E. neophidis: Ann. Appl.
Biol. (1985) 107 365376.]
erysipelas Typically, well-demarcated lesions of erythema often
affecting the face, although other areas may be involved; fever,
prostration and sepsis may occur. The causal agent is usually a
strain of Streptococcus pyogenes, and infection generally occurs
via wounds or abrasions.
(cf. ERYSIPELOID; SWINE ERYSIPELAS.)
erysipeloid A disease involving localized inflammation or CELLULITIS of skin (usually on the fingers and hands); it is caused by
Erysipelothrix rhusiopathiae and is contracted mainly by handlers of fish and meat products. Infection occurs via wounds etc.
Rarely, septicaemia or endocarditis may occur.
Erysipelothrix A genus of Gram-positive, asporogenous, nonmotile bacteria; sole species (type species): E. rhusiopathiae
(formerly E. insidiosa). Cells may be slightly curved, roundended rods (ca. 0.20.4 0.82.0 m) which form smooth,
(initially) transparent colonies (S-form), or occur mainly as
filaments (up to 60 m long) which form rough, opaque colonies
(R-form). S-forms show a strong tendency to become R-forms.
(See also PEPTIDOGLYCAN.) The organism is microaerophilic
(facultatively aerobic or anaerobic). Growth occurs at 1542 C
(optimum 37 C). Indole ve; catalase ve; urease ve; VP
ve; MR ve; H2 S +ve; aesculin not hydrolysed. In gelatin
stab cultures S-forms produce a typical pipe-cleaner (becoming
a test-tube brush) form of growth, with little or no gelatin
liquefaction. GC%: 3840.
Erysiphaceae
E. rhusiopathiae is parasitic in man, animals, birds and fish,
and can be found e.g. in animal faeces, abattoir effluents etc.
Some strains are pathogenic (see e.g. ERYSIPELOID, JOINT-ILL,
SWINE ERYSIPELAS). The organism is resistant e.g. to salting,
pickling, smoking, and low concentrations of phenol; in dried
form (e.g. in fish-meal, soil) it can remain viable for years.
[Book ref. 46, pp. 16881700.]
Erysiphaceae See ERYSIPHALES.
Erysiphales An order of homothallic and heterothallic plantparasitic fungi of the subdivision ASCOMYCOTINA (see also POWDERY MILDEWS); all species are placed in the family Erysiphaceae.
The organisms form at least partially superficial, septate
mycelium which is typically colourless and which commonly
exhibits numerous haustoria. (Dark mycelium is formed e.g.
by Sphaerotheca lanestris; cf. BLACK MILDEWS.) Ascocarp (ca.
50350 m diam.): cleistothecioid with hamathecium lacking,
often dark and rounded, and often with surface appendages;
uniascal or containing a small number of asci. Asci: bitunicate,
clavate or pyriform. Ascospores: aseptate, ellipsoidal, colourless.
Anamorphs occur e.g. in the genera Oidiopsis, Oidium and Ovulariopsis; conidia are often formed in abundance, basipetally,
on straight, unbranched conidiophores. Genera: e.g. Cystotheca,
ERYSIPHE, Leveillula, Microsphaera, Phyllactinia, Podosphaera,
Sphaerotheca, Uncinula.
[Book ref. 187.]
Erysiphe A genus of homothallic and heterothallic fungi (order
ERYSIPHALES) which include parasites and pathogens of grasses
and other plants (e.g. E. betae on beet crops, E. graminis on
cereals). Erysiphe spp form superficial mycelium on host plants;
most species form globose haustoria, but those of E. graminis
are digitate (see also TRIFORINE). The organisms give rise to darkcoloured cleistothecia. The cleistothecial surface appendages
(when present) are hypha-like, not dichotomously branched
or terminally coiled; each cleistothecium contains more than
one ascus. The ovoid to elongated conidia of E. graminis
and E. polygoni are highly vacuolated; the conidiophores of
E. graminis are distinctive in that in each the basal cell is slightly
swollen. Conidia germinate by a germ tube which forms an
appressorium.
erythema Redness of the skin due e.g. to INFLAMMATION or
infection.
erythema infectiosum (fifth disease; slapped cheek syndrome) A
benign, infectious disease, affecting mainly children, characterized
by exanthem which begins on the face and gives a slapped cheek
appearance. The causal agent is parvovirus B19. (cf. EXANTHEM
SUBITUM.)
erythema nodosum leprosum See LEPROSY.
erythrasma A chronic skin infection caused by Corynebacterium
minutissimum. The reddish-brown lesions occur in the groin and
armpits and fluoresce coral-pink under Woods lamp.
erythritol The POLYOL corresponding to erythrose. It occurs e.g.
in certain fungi, particularly in the Ustilaginales and Agaricales
(where it apparently functions as a storage carbohydrate), and
as a major photosynthetic product in certain unicellular and
filamentous green algae (e.g. Phycopeltis, Trentepohlia). It can
be metabolized e.g. by many yeasts.
Erythrobacter A genus of Gram-negative, aerobic, halophilic,
ovoid to rod-shaped, orange- or pink-pigmented bacteria which
are motile by subpolar flagella. The cells contain bacteriochlorophyll a which is synthesized only under aerobic conditions
(cf. RHODOSPIRILLALES). Metabolism appears to be chemoorganotrophic (mainly respiratory); autotrophic growth does not occur.
Strains have been isolated from seaweeds growing near high-tide
Escherichia
B19 has been cultured in the erythroid cells from human bone
marrow and fetal liver; in vitro propagation of the virus depends
on the presence of the hormone erythropoietin (which is specific
to erythroid cells). The cell-surface receptor for B19 is the red
cell P antigen (globoside a tetrahexose ceramide), the virus
binding with high affinity to the carbohydrate moiety. P antigen
is expressed e.g. on erythroid progenitors, mature red cells,
megakaryocytes, endothelial cells and heart cells. (Individuals
with the rare p phenotype, who do not express P antigen, are
not susceptible to B19.)
Viral replication is dependent on mitotically active cells, the
virus being highly tropic for human erythroid cells in the late S
phase of the cell cycle.
B19 DNA can be demonstrated in the nasal secretions of
individuals with B19 viraemia, and the respiratory route is
believed to be important in virus transmission. Infection can
also be transmitted via blood and blood products.
Clinical manifestations of infection appear to depend primarily
on host factors such as immunocompetence. In immunocompetent persons with a normal erythroid turnover, infection may lead
to a short-term (48 days) halt in red cell production without development of anaemia. However, given a high turnover
of red cells, even a temporary loss of red cell production may
bring about an aplastic crisis. In immunocompromised patients
infection may lead to chromic anaemia. In the fetus, infection
may result e.g. in HYDROPS FETALIS. Other manifestations of B19
infection include arthralgia and rash. (See also ERYTHEMA INFECTIOSUM.)
Among adults, seroprevalence of B19 IgG antibody is high,
and the proportion of seropositives increases with age; IgG
antibody develops within 2 weeks of infection and persists
for life.
[Persistent B19 infection: RMM (1995) 6 246256. Molecular epidemiology of parvovirus B19: RMM (1997) 8 2131.
Haematological consequences of parvovirus B19 infection: BCH
(2000) 13 245259.]
ES1ES21 proteins See RIBOSOME.
ESAT-6 A 6 kDa secreted protein (early secreted antigenic
target) encoded by Mycobacterium tuberculosis and by M. bovis
and M. africanum (members of the M. tuberculosis complex)
but apparently not encoded by any of the (vaccine) strains of
M. bovis BCG. (The operon encoding ESAT-6 is also reported
to encode a novel, low-molecular-weight protein which has been
designated CFP-10 [Microbiology (1998) 144 31953203].)
Yet another secreted protein, MPT64, appears to be encoded
by all strains of M. tuberculosis and BCG Tokyo but not
by strains of BCG Danish 1331 [BCID (1997) 4 157172
(167168)].
Antigens such as ESAT-6 may be useful e.g. in SKIN TESTS
for distinguishing between sensitization due to (i) tubercle
bacilli, (ii) vaccination strains of BCG, or (iii) environmental
mycobacteria (cf. TUBERCULIN TEST).
A test using ESAT-6 has been compared with a PPDbased test for the diagnosis of bovine tuberculosis; ESAT6 was associated with a lower sensitivity but with increased
specificity useful e.g. for testing in areas which have a low
incidence of tuberculosis [VR (2000) 146 659665].
The specificity of ESAT-6 for the M. tuberculosis complex
has been exploited (by means of an ex-vivo ELISPOT ASSAY) for
the enhanced tracing of contacts in epidemiological studies on
human tuberculosis [Lancet (2001) 357 20172021].
ESBLs Extended-spectrum b-LACTAMASES.
esc genes See PATHOGENICITY ISLAND.
eschar Dead tissue which separates (sloughs) from the underlying living tissue. An eschar is formed e.g. in SCRUB TYPHUS.
Escherichia A genus of Gram-negative bacteria of the family
ENTEROBACTERIACEAE (q.v. for general features); in molecular
taxonomy, Escherichia is placed in the gamma group of the
Proteobacteria. GC% 50. Type species: E. coli.
E. coli has long been the principal guinea pig of the
microbiologist, and has been studied more extensively than any
other species. (Nevertheless, E. coli should not be regarded as
the typical bacterium; the great diversity of bacteria makes
such a concept meaningless.) The following refers specifically
to E. coli (other species are mentioned at the end of the entry).
Cells are typically straight, round-ended rods, ca. 0.50.8
14 m, normally occurring singly or in pairs; they stain well
with ANILINE DYES.
The cell has a typical Gram-negative-type CELL WALL consisting of an OUTER MEMBRANE and a layer of PEPTIDOGLYCAN. The
CYTOPLASMIC MEMBRANE contains e.g. various TRANSPORT SYSTEMS, energy-converting systems and chemosensors as well as
components of osmoregulatory systems (see OSMOREGULATION);
the latter include MECHANOSENSITIVE CHANNELS [mechanosensitive channels in E. coli : ARP (1997) 59 633657], aquaporins
and glycerol facilitators (see MIP CHANNELS).
Cells are typically motile (peritichously flagellate) [second
flagellar system in E. coli. JB (2005) 187 14301440]. FIMBRIAE
are usually present. Type I fimbriae (the most common type) may
be suppressed by P FIMBRIAE (q.v.).
Some cells have a CAPSULE or microcapsule (see e.g. COLANIC
ACID, COLOMINIC ACID; cf. TEICHOIC ACIDS).
Numerous strains of E. coli are distinguished serologically (on
the basis of their O ANTIGENS, H ANTIGENS and K ANTIGENS), or by
PHAGE TYPING, colicin typing, antibiotic-resistance patterns etc.
E. coli exhibits CHEMOTAXIS; the Tsr protein (an MCP in
chemotaxis) may also function as a pmf-dependent sensor in
aerotaxis [PNAS (1997) 94 1054110546]. [Ecological role of
energy taxis: FEMS Reviews (2004) 28 113126.]
The chromosome (cccDNA) is about 4.7 million base-pairs in
length. [Complete sequence: Science (1997) 277 14531474.]
Replication occurs by the Cairns-type mechanism (bidirectionally from the origin, oriC ). [Localization of chromosomal segments during the cell cycle: GD (2000) 14 212223.] There are
several systems for DNA REPAIR. (See also SOS SYSTEM.)
Many of the genes occur within OPERONS which may encode
e.g. metabolic enzymes and/or components of TRANSPORT SYSTEMS (e.g. LAC OPERON).
TRANSCRIPTION of most genes involves the SIGMA FACTOR s70 ;
other sigma factors include s32 (see HEAT-SHOCK PROTEINS). A
proportion of mRNA transcripts are polyadenylated at the 3
end [characterization of the E. coli poly(A)polymerase: NAR
(2000) 28 11391144].
Gene transfer can occur in vivo by CONJUGATION or TRANSDUCTION. Competence in TRANSFORMATION can be induced in the
laboratory in ice-cold solutions of calcium chloride [possible
mechanism: JB (1995) 177 486490]. High-efficiency transformation can be achieved by ELECTROPORATION [NAR (1999) 27
910911].
Metabolism is respiratory under aerobic conditions (see RESPIRATION). FERMENTATION (sense 1) or ANAEROBIC RESPIRATION
occurs anaerobically. Glucose, mannitol and various other substrates are taken up by the PTS (q.v.). Lactose is taken up by
protonlactose symport, and melibiose by Na+ /melibiose symport (see SODIUM MOTIVE FORCE). Glucose is fermented (usually
aerogenically) by a MIXED ACID FERMENTATION (cf. ALKALESCENSDISPAR GROUP).
287
escN gene
estB gene See ETEC.
ET EPIDERMOLYTIC TOXIN.
h-value (of a disinfectant) See DILUTION COEFFICIENT.
etamycin Syn. VIRIDOGRISEIN.
etanercept See TNF.
ETC ELECTRON TRANSPORT CHAIN.
ETEC Enterotoxigenic Escherichia coli: strains of E. coli which
adhere to the small intestine in man and/or animals and
form heat-labile ENTEROTOXIN (LT-I/LT-II: inactivated at
60 C/30 min) and/or heat-stable enterotoxin (ST-I/ST-II: not
inactivated at 100 C/30 min). Strains of ETEC cause mild to
severe (cholera-like) diarrhoea in humans of all ages and/or
similar disease in animals. (See also COLIBACILLOSIS and FOOD
POISONING; cf. EAGGEC, EIEC, EHEC and EPEC.)
The ability to adhere to (i.e. colonize) the small intestine
crucial for virulence involves various plasmid-encoded FIMBRIAE. Strains from humans have non-fimbrial and fimbrial colonization factors, e.g. CS6 and colonization factor antigens
CFAI (F2) and CFAII (F3); CFAII has three components: CS1,
CS2 and CS3 (CS = coli surface). Strains of ETEC from animals have e.g. K88 or K99 FIMBRIAE (see also F6 FIMBRIAE).
[Fimbriae of human strains of ETEC and their possible use in
vaccines: RMM (1996) 7 165177.]
LT-I closely resembles the CHOLERA TOXIN in structure: both
toxins have the AB5 arrangement of subunits (found also e.g.
in SHIGA TOXIN), and there is an 80% homology in amino
acids. LT-I and CT cross-react antigenically, and they also have
similar binding sites and a common mode of action; however,
for unknown reasons, disease produced by LT-I is generally less
severe, and of shorter duration, than that due to CT.
LT-II occurs e.g. in pigs, rarely in humans. The A subunit
is <60% homologous to that of LT-I, and the B subunits are
essentially non-homologous (so that the binding site differs);
the basic mode of action is similar to that of LT-I [MR (1996)
60 167215 (pp 191, 192)].
Genes encoding the LT toxins are carried on Ent plasmids.
ST-I (= STa) is a (methanol-soluble) peptide containing 18
or 19 amino acids produced from a 72-amino-acid precursor;
following cleavage, three disulphide bonds are catalysed in the
peptide by the protein DsbA prior to secretion. ST-I binds to
receptors in the brush border membrane; the receptors have
guanylate cyclase activity, and binding by ST-I activates the
cyclase leading to increased levels of intracellular cyclic GMP
that apparently stimulate secretion of chloride and/or inhibit
the absorption of NaCl. The net result is believed to be
secretion of fluid into the gut. An alternative view of the mode
of action of this toxin involves interruption of the luminal
acidification mechanism (apparently through inhibition of the
Na+ /H+ exchanger in the brush border membrane) leading to
a reduction in the absorption of fluid [JAM (2001) 90 726].
Interestingly, the receptor sites for ST-I are the same as those
used by guanylin an endocrine hormone (a peptide of 15
amino acid residues) whose normal function apparently involves
regulation of NaCl and water homeostasis in the gut. (The
number of receptor sites has been reported to decrease with
age infants having a large number of receptors; this may give
a reason for the increased severity of diarrhoea in infants and
young children with ST-I infection.) [MR (1996) 60 167215
(pp 190, 191); MP (1998) 24 123131.]
ST-II (STb) is a (methanol-insoluble, trypsin-sensitive)
polypeptide containing 48 amino acid residues (derived from
a precursor of 71 amino acid residues). The toxin does not
cause secretion in the small intestine of mice or rats owing to its
HJARRES
DISEASE; MENINGITIS; OEDEMA DISEASE; OSTEOMYELITIS;
PNEUMONIA; URINARY TRACT INFECTION.)
[PCR-based detection of E. coli O157: JCM (1998) 36
18011804.]
[Target genes for virulence assessment of Escherichia coli
isolates from food, water and the environment: FEMS Reviews
(2000) 24 107117.]
Other species within the genus. E. blattae is an apparently
harmless commensal in the hindgut of the cockroach (Blatta
orientalis). Test reactions: indole ve; malonate +ve; lactose
ve.
Other proposed species include E. fergusonii [JCM (1985) 21
7781], E. hermanii [JCM (1982) 15 703713] and E. vulneris
[JCM (1982) 15 11331140].
escN gene See PATHOGENICITY ISLAND.
esculin Syn. AESCULIN.
Es An RNA POLYMERASE holoenzyme.
espA gene See PATHOGENICITY ISLAND.
espB gene See PATHOGENICITY ISLAND.
EspB protein See PROTEIN SECRETION (type III systems).
espE gene See PATHOGENICITY ISLAND.
EspE protein See PROTEIN SECRETION (type III systems).
espundia See MUCOCUTANEOUS LEISHMANIASIS.
ESR ELECTRON SPIN RESONANCE.
estA gene See ETEC.
established cell line (continuous cell line) A population of
cells derived either from a tumour, or from a TISSUE CULTURE
following transformation which appears to be capable of
unlimited in vitro propagation. See e.g. BHK-21, BS-C-1, DETROIT-6,
HELA, HEP-2, VERO and WISH.
288
Eubacterium
inactivation by trypsin. It is apparently without effect on human
intestine under in vitro (USSING CHAMBER) conditions; strains
secreting ST-II are infrequently involved in human disease. The
mode of action is unknown but apparently does not involve
cyclic nucleotides (i.e. the mode of action differs from that of
ST-I). [ST-II: Microbiology (1997) 143 17831795.]
ST-I is encoded by estA a plasmid-borne gene located
within a transposon (Tn1681 ). ST-II is encoded by the plasmidborne gene estB.
[Heat-stable enterotoxin associated with resistance to colon
cancer: PNAS (2003) 100 26952699.]
ETEC strains commonly belong to serogroups O6, O8, O15,
O25, O27, O63, O78, O115, O148, O153 and O159.
ethambutol (Myambutol) A synthetic drug, d-(2,2 -(ethylene
diimino)-di-1-butanol), used (e.g. in combination with ISONIAZID)
in the treatment of TUBERCULOSIS; it inhibits growing cells of
Mycobacterium tuberculosis and M. bovis. Major adverse effects
include optic neuritis and a loss of the ability to discriminate
red/green (particularly in patients on a high-dose regimen)
[BCID (1997) 4 5354].
ethanol (as an antimicrobial agent) See ALCOHOLS.
ethanol fermentation See ALCOHOLIC FERMENTATION and INDUSTRIAL ALCOHOL.
ethazole (5-ethoxy-3-trichloromethyl-1,2,4-thiadiazole) An agricultural systemic ANTIFUNGAL AGENT used e.g. as a seed dressing
for protection against Pythium, Phytophthora and Rhizoctonia.
ethidium bromide (2,7-diamino-10-ethyl-9-phenylphenanthridinium bromide) A trypanocidal, bacteriostatic dye. It is an
INTERCALATING AGENT (f = 26 ) which inhibits transcription
and DNA replication; it binds specifically to dsDNA (or to
base-paired regions of ssDNA) with no apparent preference
for particular base sequences. In eukaryotes it is highly selective for mtDNA and kinetoplast DNA. Ethidium bromide can
induce nuclease attack and (non-enzymic) photochemical nicking of DNA.
Owing to their limited capacity to unwind, small cccDNA
molecules can bind less ethidium bromide than can equivalent
linear or nicked DNAs, and hence show a smaller reduction in
density in the presence of ethidium bromide; this is exploited in
methods for separating ccc from linear/nicked DNA by isopycnic
ultraCENTRIFUGATION.
ethirimol (5-n-butyl-2-ethylamino-4-hydroxy-6-methylpyrimidine;
trade names: e.g. Milstem, Milgo) A HYDROXYPYRIMIDINE ANTIFUNGAL AGENT which is used as a seed dressing and as a foliar
spray for the control of powdery mildews in cereals; it also
controls powdery mildew in e.g. sugar beet.
ethyl stibamine See ANTIMONY.
ethylene (plant pathol.) A PHYTOHORMONE which, in higher
plants, can induce e.g. germination, flowering, fruit ripening,
senescence depending on the plant and its stage of development. Ethylene is also produced by plant tissues in response to
stress, damage, or infection by certain pathogens, and large quantities are produced by plant tissues exhibiting HYPERSENSITIVITY;
it may give rise to certain symptoms of diseasee.g. EPINASTY,
premature ripening of fruit or leaf-fall.
ethylene glycol See ALCOHOLS.
ethylene oxide A colourless, highly reactive, water-soluble cyclic
ether (b.p. 10.8 C) used (as a vapour) for the DISINFECTION or
STERILIZATION of e.g. medical equipment and certain heat-labile
materials. The vapour forms explosive mixtures with air in a
wide range of proportions and is commonly diluted with carbon
dioxide, nitrogen or fluorohydrocarbons: e.g. Carboxide contains
10% ethylene oxide, 90% CO2 (see also e.g. CRYOXICIDE,
289
Eubenangee subgroup
euglenoid flagellates (euglenids; euglenoids) A group of unicellular organisms regarded either as algae (class Euglenophyceae,
division Euglenophyta) or as protozoa (see PHYTOMASTIGOPHOREA). The vegetative cell has no cell wall, but has a pellicle
consisting of spirally arranged, interlocking, proteinaceous strips
beneath the plasmalemma. The pellicle may be flexible (in e.g.
Astasia, Distigma and EUGLENA) or rigid (in e.g. Menoidium,
PHACUS and Rhabdomonas). Mucilage-secreting muciferous bodies occur in helical rows beneath the pellicle. In some genera
(e.g. Klebsiella, TRACHELOMONAS) the cell is partly or totally
enclosed in a mineralized LORICA. At the anterior end of the cell
is an invagination, the reservoir (also called the gullet although
it does not function in feeding), which opens to the exterior via a
narrow canal. A contractile vacuole commonly empties into the
reservoir. In most genera two flagella arise from basal bodies
at the base of the reservoir, but in some genera (e.g. Astasia,
Colacium, Euglena, Phacus) only one flagellum (containing a
PARAXIAL ROD) actually emerges from the cell via the canal; in
e.g. Distigma, Eutreptia, PERANEMA and HETERONEMA two flagella are emergent, one of which is directed anteriorly, the other
laterally or posteriorly. (Parasitic euglenids may have 3 or more
emergent flagella.)
Many euglenids are photosynthetic, possessing green chloroplasts containing chlorophylls a and b and various carotenoids.
However, photosynthetic species can apparently also grow heterotrophically on e.g. acetate or ethanol in the dark, and many
genera (e.g. Astasia, Khawkinea, Rhabdomonas) are colourless
and obligately heterotrophic; PERANEMA and related genera are
holozoic. A storage compound characteristic of both photosynthetic and heterotrophic euglenids is PARAMYLON.
Euglenids reproduce chiefly by longitudinal binary fission;
MITOSIS occurs within the nuclear membrane and does not
involve a spindle. Palmelloid phases are common in some
species. (cf. COLACIUM.) Desiccation-resistant cysts are formed
in e.g. Distigma and Euglena under adverse conditions. Sexual
reproduction is virtually unknown.
Euglenoid flagellates are mainly free-living aquatic organisms,
occurring in fresh water (e.g. most Euglena spp, Phacus) or
in brackish or sea water (e.g. some Euglena spp, Eutreptia,
Klebsiella). Some species are parasitic (e.g. Euglenamorpha in
the gut of tadpoles).
euglenoid movement See EUGLENA.
Euglenophyceae See EUGLENOID FLAGELLATES.
Euglypha A genus of testate amoebae (order Gromiida, class
FILOSEA) in which the test (ca. 30160 m diam.) is composed
of siliceous scales which are synthesized within the cytoplasm
before incorporation into the test. Pseudopodia are generally narrow, filamentous, and sometimes anastomosing. Species occur in
fresh water, activated sludge, anaerobic regions in acidic bogs,
etc. (cf. PAULINELLA.)
eugonic Refers to a strain of e.g. Mycobacterium which, on
culture, produces growth which is more luxuriant than that
produced by other (dysgonic) strains; the growth itself may also
be described as eugonic (or dysgonic).
eugregarines See GREGARINASINA.
eukaryote (eucaryote) A type of CELLULAR (sense 2 or 3) organism in which the CHROMOSOMES are separated from the cytoplasm
by a membrane (see NUCLEUS) and usually contain HISTONES (cf.
DINOFLAGELLATES); the CYTOPLASMIC MEMBRANE contains sterols;
mitochondria are commonly present; chloroplasts occur in photosynthetic species; RIBOSOMES in the cytoplasm are of the 80S
type; the CELL WALL (when present) contains e.g. CELLULOSE
or CHITIN; storage compounds apparently never include poly-bhydroxybutyrate; flagella or cilia (when present) are structurally
excipulum
relatively complex (see FLAGELLUM (b) and CILIUM). Eukaryotic
MICROORGANISMS include ALGAE, FUNGI, LICHENS and PROTOZOA.
Eukaryotes may have arisen some 23.5 billion years ago
[Science (1996) 271 470477] from an energy-based symbiotic
relationship between cells of the ARCHAEA and BACTERIA [the
hydrogen hypothesis: Nature (1998) 392 3741].
(cf. PROKARYOTE.)
eumycetoma See MADUROMYCOSIS.
Eumycetozoa See EUMYCETOZOEA.
Eumycetozoea According to one protozoal classification scheme
[JP (1980) 27 3758]: a class of SLIME MOULDS of the RHIZOPODA. Members of the class typically form myxamoebae with
filose pseudopodia or subpseudopodia; flagella, when formed,
lack mastigonemes. Aerial fruiting bodies are produced. Subclasses: Protosteliia (equivalent to the PROTOSTELIOMYCETES
together with CERATIOMYXA); Dictyosteliia (equivalent to the
DICTYOSTELIOMYCETES); Myxogastria (equivalent to the MYXOMYCETES). According to another classification scheme [Book
ref. 147, pp. 45], equivalent taxa are the class Eumycetozoa
(subphylum MYCETOZOA) and its constituent subclasses Protostelia, Dictyostelia and Myxogastria.
Eumycota In some mycological classification schemes [e.g.
Book ref. 64]: a division which includes the true fungi (subdivisions ASCOMYCOTINA, BASIDIOMYCOTINA, DEUTEROMYCOTINA,
MASTIGOMYCOTINA and ZYGOMYCOTINA). (cf. MYXOMYCOTA.)
Euphorbia mosaic virus See GEMINIVIRUSES.
euphotic zone See PHOTIC ZONE.
euploid (1) Having the basic haploid number of chromosomes
or any exact multiple of the haploid number. (cf. ANEUPLOID.)
(2) Having a chromosome complement characteristic of the
species. (cf. HETEROPLOID.)
Euplotes
A genus of highly evolved ciliate protozoa (order
HYPOTRICHIDA); species occur in freshwater, brackish and marine
habitats, and some (e.g. E. moebiusi ) are common in some
SEWAGE TREATMENT plants. Cells: roughly ovoid, ca. 50150 m
in length, with a flattened ventral side and a dorsal side
which is often markedly ridged; the cytostome is anterior and
ventral, the distal part of the AZM forming a conspicuous,
protruding fringe. The ventral surface carries a number of cirri
which occur in localized groups and on which the organism
is capable of creeping or walking movements; other forms
of somatic ciliature are absent. The macronucleus is typically
band-like and curved, the micronucleus small and spherical.
[Macronuclear development in E. crassus: JCB (1985) 101
7984.] Some strains contain endosymbionts (see OMICRON). A
contractile vacuole is present. Asexual reproduction occurs by
binary fission. CONJUGATION occurs (see SYNGEN). TRANSLATIONAL
FRAME-SHIFTING seems common [Cell (2002) 111 763766].
Food: algae, bacteria, other protozoa.
European bat lyssavirus See LYSSAVIRUS.
European blastomycosis Syn. CRYPTOCOCCOSIS.
European foulbrood A BEE DISEASE which affects larvae (ca.
45 days old) of Apis mellifera and A. cerana; infected larvae
die, turn brown and putrefy. The causal agent is Melissococcus
pluton (formerly called Streptococcus pluton) [JAB (1983) 55
6569]; infection occurs by ingestion, and the bacteria multiply
within and sometimes fill the midgut. Secondary invaders
may include e.g. Enterococcus faecalis and Bacillus alvei. (cf.
AMERICAN FOULBROOD.)
European swine fever Syn. SWINE FEVER.
Eurotiales An order of mainly saprotrophic fungi of the subdivision ASCOMYCOTINA; anamorphs occur e.g. in the genera ASPERGILLUS and PENICILLIUM. Ascocarp: cleistothecioid,
excipulum proprium
excipulum proprium See PROPER MARGIN.
excipulum thallinum See THALLINE MARGIN.
excision repair Any DNA REPAIR process which can repair lesions
affecting only a single strand of dsDNA (not, for example, interstrand cross-linking) and which involves removal and replacement of one or more nucleotides. Excision repair in Escherichia
coli can be considered under three main headings:
(i) BASE EXCISION REPAIR, i.e. repair of an AP SITE after preliminary cleavage of a base (see ADAPTIVE RESPONSE and URACIL-DNA
GLYCOSYLASE).
(ii) MISMATCH REPAIR, used mainly for errors that escape proofreading during DNA replication.
(iii) UvrABC-mediated repair (nucleotide excision repair;
short patch repair). This common excision repair mechanism
recognizes and repairs DNA which has been damaged/distorted
by ultraviolet radiation or by certain other causes; damage may
consist e.g. of a thymine dimer or a Pyr(6-4)Pyo photoproduct (see ULTRAVIOLET RADIATION). The ATP-dependent enzyme
system UvrABC (also called ABC excinuclease) consists of
three proteins encoded by genes uvrA, uvrB and uvrC. Initially a UvrA dimer binds to the damaged DNA. UvrB then
binds to the dimer, and the complex UvrA2 B translocates to the
precise site of damage; such translocation is apparently ATPdependent (the zinc-binding protein UvrA being an ATPase).
UvrC displaces UvrA, and the UvrBC complex nicks the damaged strand on either side of the lesion, the 3 nick being made
first. UvrD (= helicase II) then displaces UvrC together with
the short sequence of nucleotides containing the site of damage. DNA polymerase I fills the single-stranded gap, displacing
UvrB, and the repair is completed by a ligase. In E. coli only
about 10 nucleotides in and around the damaged site are excised
(thus accounting for the name short patch repair). (See also
PHOTOLYASE.)
The UvrABC system is enhanced during the SOS RESPONSE.
Another repair system, the so-called error-prone repair system
(involving translesion synthesis of DNA), appears to operate
only during the SOS RESPONSE (q.v.).
excisionase See e.g. BACTERIOPHAGE l.
exciter filter See MICROSCOPY (e).
exclusion limit See PORIN.
exclusion zone See MICROTUBULES.
exconjugant A cell which has separated from another following
CONJUGATION.
excystation Syn. EXCYSTMENT.
excystment (excystation) The release of one or more vegetative
(or other) cells from a CYST.
exergonic reaction Any reaction which is accompanied by the
liberation of energy. (cf. ENDERGONIC REACTION.)
exflagellation See PLASMODIUM.
exfoliatin Syn. EPIDERMOLYTIC TOXIN.
Exidia See TREMELLALES.
Exiguobacterium A genus of Gram-positive, asporogenous, facultatively anaerobic, rod-shaped or coccoid, motile bacteria
[JGM (1983) 129 20372042]. E. aurantiacum is an ALKALOPHILE which has been isolated from potato processing effluent.
exine See CYST (a).
Exo Abbr. for exonuclease; for example, Exo III is EXONUCLEASE III.
Exobasidiales An order of plant-endoparasitic, characteristically
GALL-inciting fungi (subclass HOLOBASIDIOMYCETIDAE) which
form hymenia that emerge through the epidermis in parasitized
plants. Genera include Exobasidium (see also BLISTER BLIGHT)
and Kordyana. (cf. BRACHYBASIDIALES.)
extrusome
extracytoplasmic oxidation In certain bacteria: the oxidation of
a substrate at the external face of the cytoplasmic membrane,
or within the periplasmic region, giving rise to (or augmenting) a proton motive force (pmf: see CHEMIOSMOSIS). During
such oxidations, protons formed at the extracytoplasmic site
contribute to pmf, while electrons (derived from the substrate)
pass through the cytoplasmic membrane (a process sometimes
called vectorial electron transfer) and are involved in electronand proton-consuming reactions. [Early review: MR (1985) 49
140157.]
Substrates oxidized extracytoplasmically include e.g. (depending on species): hydrogen, formate, methanol, glucose and various ions particularly ferrous ions. Intracellular terminal electron acceptors include e.g. oxygen, fumarate, sulphate ions and
nitrate ions.
Oxidations carried out extracytoplasmically include e.g. the
oxidation of hydrogen by Desulfovibrio spp, Escherichia coli
and by those HYDROGEN-OXIDIZING BACTERIA containing an NADindependent membrane-bound HYDROGENASE. In E. coli the
hydrogenase is located on the external surface of the cytoplasmic
membrane, while in Desulfovibrio spp a soluble hydrogenase is
located in the periplasmic region.
In Beggiatoa, sulphide appears to be oxidized extracytoplasmically to elemental sulphur. It has been proposed that
Thiobacillus thiooxidans can oxidize insoluble (colloidal) sulphur extracytoplasmically.
In Thiobacillus ferrooxidans, the oxidation of ferrous to ferric
ions occurs extracytoplasmically; it appears to involve e.g. an
oxidase, c-type and a-type cytochromes and RUSTICYANIN [see
e.g. MR (1994) 58 3955 (4748)].
In some bacteria, ions such as Mn2+ or U4+ may be oxidized
extracytoplasmically.
Some bacteria (e.g. Pseudomonas aeruginosa) can generate pmf by extracytoplasmic oxidation of glucose to gluconate
by glucose dehydrogenase (a QUINOPROTEIN) [JB (1985) 163
493499]; in these organisms the enzyme glucose dehydrogenase, with its cofactor pyrroloquinoline quinone (PQQ), occurs
on the outer surface of the cytoplasmic membrane. The gluconate formed can then be transported across the membrane,
phosphorylated to 6-phosphogluconate, and fed into the ENTNERDOUDOROFF PATHWAY.
E. coli (and some related bacteria) normally form a
membrane-bound glucose dehydrogenase which lacks the
cofactor (PQQ); such organisms can carry out extracytoplasmic
oxidation only if they are supplied with exogenous PQQ [IJSB
(1989) 39 6167]. However, a mutant strain of E. coli with a
non-functional PTS system is able to synthesize PQQ and to carry
out extracytoplasmic oxidation; this has suggested that PQQencoding genes are normally present but not expressed [JGM
(1991) 137 17751782].
extranuclear genes Syn. CYTOPLASMIC GENES.
extravasation See INFLAMMATION.
extremophile See ARCHAEA.
extrinsic allergic alveolitis (EAA; hypersensitivity pneumonitis)
A form of pneumonitis, which appears to involve an ARTHUS-TYPE
REACTION and a DELAYED HYPERSENSITIVITY (type IV) reaction,
caused by the inhalation of certain allergen(s). Examples of
EAA include e.g. BAGASSOSIS, CHEESE-WASHERS LUNG, FARMERS
LUNG, MAPLE BARK STRIPPERS DISEASE, SUBEROSIS. [CIA (1984) 4
173192.]
extrusome A generic term for an extrusile organelle (function
often unknown), various types of which occur near the cell
surface in many ciliates and in some other organisms. Examples:
exudative dermatitis
haptocyst, kinetocyst (see
rhabdocyst, TOXICYST, TRICHOCYST (cf.
polar filament in MICROSPOREA and MYXOSPOREA).
exudative dermatitis Syn. GREASY PIG DISEASE.
EYA See EGG-YOLK AGAR.
eye microflora The surface of the eye and the conjunctival membranes normally bear only a sparse microflora owing to the
constant flushing action of the secretions of the lacrimal glands;
these secretions contain certain antimicrobial agents e.g.
LACTOFERRIN, LYSOZYME, and immunoglobulins (see IGA). Organisms which may be isolated from the eye surfaces include certain
members of the SKIN MICROFLORA, e.g. staphylococci. (See also
BODY MICROFLORA and CONJUNCTIVITIS.)
eyepiece micrometer See MICROMETER.
eyespot (1) (stigma) In certain algae: a body consisting of a
group, layer or layers of closely-packed lipid globules which,
according to species, occurs within the CHLOROPLAST (e.g. in
members of the Chlorophyta) or outside it (e.g. in euglenoid
flagellates). In most or all cases an eyespot contains orange
or red CAROTENOID pigments. In certain dinoflagellates (e.g.
conocyst,
EJECTOSOME, FIBROCYST,
AXOPODIUM), PEXICYST,
294
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
F
f. See FORMA SPECIALIS.
F Phenylalanine (see AMINO ACIDS).
F-actin See ACTIN.
F antigens Fimbrial antigens see FIMBRIAE. (cf. K ANTIGENS.)
F+ donor See F PLASMID.
F-duction See SEXDUCTION.
F factor See F PLASMID.
F layer See CYANOBACTERIA (section II).
F-like pili See PILI.
F pili See PILI.
F plasmid (formerly F factor, fertility factor) An IncFI PLASMID which occurs e.g. in Escherichia coli with a COPY NUMBER of usually 1 or 2; it consists of a ccc dsDNA molecule
(ca. 95 kilobases) which includes two copies of the INSERTION
SEQUENCE IS3, one each of IS2 and IS1000, and sequences relating to replication, incompatibility and CONJUGATION (sense 1b).
An F plasmid confers on the host cell the characteristics of a
conjugal donor, and it can also affect the cells phenotype in
other ways: see e.g. FEMALE-SPECIFIC PHAGE. (See also PIF.)
Within the host cell, an F plasmid exists either in the
autonomous (extrachromosomal) state, i.e. as a free, circular
plasmid, or integrated in the hosts chromosome. (cf. EPISOME.)
Integration occurs by homologous RECOMBINATION between an
insertion sequence in the plasmid and one in the chromosome
(see CAMPBELL MODEL); copies of insertion sequences IS2 and
IS3 are common in the chromosome of E. coli. An integrated F
plasmid may undergo aberrant excision from the chromosome:
see PRIME PLASMID.
Conjugation mediated by the F plasmid. The F plasmid can
mediate conjugation either in the autonomous state or in the
integrated state.
In the autonomous (extrachromosomal) state an F plasmid can
efficiently promote its own intercellular transfer by CONJUGATION
(sense 1b). A cell containing an autonomous F plasmid is called
an F+ donor, while a cell lacking an F plasmid (but able to
receive one by conjugation) is called an F recipient. (Such
cells are sometimes referred to as male and female cells,
respectively.) In a mixed population of F+ and F cells, a copy
of the F plasmid is transferred at high frequency, i.e. all, or
nearly all, of the F cells receive a copy (and hence become
F+ donors themselves); in such F+ F crosses, chromosomal
genes are usually not transferred.
Integration of an F plasmid into the chromosome gives rise
to an HFR DONOR (q.v.) in which the chromosome is mobilized
for transfer by the integrated plasmid (see CONJUGATION).
Whether conjugation is mediated by an autonomous or
integrated F plasmid, the mechanism of transfer depends on an
extensive (ca. 33 kilobase) region of the plasmid the transfer
region containing over 30 genes. This region is commonly
referred to as the transfer operon, although it contains more
than one promoter; however, most of the tra genes are found
in a single large operon (traYI ). The traJ and traM genes
(both located immediately downstream of oriT ) are outside the
traYI operon; traJ has one promoter, traM has two. traY, the
first gene of the traYI operon, is adjacent to traJ. The traYI
operon is transcribed by the Es70 holoenzyme; activation of the
traY promoter is dependent on TraJ, but other factors appear to
be needed for full activation. Apparently some genes within the
traYI operon (e.g. traS, traT ) have their own promoters, and
their expression seems to be independent of TraJ.
About 15 genes are needed for synthesis and assembly of
the F pilus. The traA gene encodes the precursor molecule
that is processed to form the subunit, pilin, from which PILI
are assembled; the initial product of traA (MWt ca. 13000) is
processed to a final size of MWt ca. 7000. Genes traQ and traX
are reported to be involved in processing the traA gene product.
Products of the traG and traN genes have been associated
with stabilization of donorrecipient mating contacts.
The traI gene product is a HELICASE which is needed for siteand strand-specific nicking at oriT (the origin of transfer) and
for unwinding DNA during conjugal transfer [JBC (1991) 266
1623216237].
The traM gene product has binding sites in the oriT region
(one of which, sbmC, is associated with DNA transfer); it is
also linked with the cytoplasmic membrane, possibly via TraD.
The role of TraM in conjugation has not been clarified, but
it is apparently essential for transfer of DNA. In a related
IncF plasmid (R1), TraM stimulated nicking at oriT by TraI
[JMB (1998) 275 8194]; in the F plasmid, TraY and the
INTEGRATION HOST FACTOR were reported to stimulate nicking at
oriT in vitro [JBC (1995) 270 2837428380]. TraM may have
a role in relaying the (currently unknown) mating signal on
establishment of stable cellcell contact.
The products of traS and traT are involved in SURFACE
EXCLUSION.
traM is autoregulated but needs TraY for full expression;
expression is affected by external factors, and is negligible in
stationary phase cells. Most genes in the traYI operon are positively regulated by TraJ, and in most IncF plasmids, expression
of traJ is under negative control of the FINOP SYSTEM (q.v.) so
that the transfer genes are normally repressed. The F plasmid
lacks a functional finO gene, i.e. in this particular plasmid, traJ
is not under negative control; consequently, the transfer genes
are constitutively derepressed (that is, permanently switched
on). (See also FERTILITY INHIBITION.)
[Control of transfer genes in F-like transfer systems: FEMS
Reviews (1998) 21 291319 (291295).]
Replication of the F plasmid. In wild-type F plasmids replication occurs bidirectionally from an origin and is under stringent
control (see PLASMID). The F plasmid has two origins of replication: oriV (= ori 1) and oriS (= ori 2); in wild-type F plasmids,
a PRIMOSOME assembly site is present near ori 2 [PNAS (1983)
80 71327136]. (In MINI-F PLASMIDS containing both origins,
replication occurs preferentially, and bidirectionally, from ori1.)
Host factors needed for F plasmid replication include the products of genes dnaB, dnaC and dnaE ; replication of the plasmid
is independent of the dnaA product. (See also INTEGRATIVE SUPPRESSION.)
Control of replication involves the (plasmid-encoded) RepE
protein (= E protein). Molecules of the E protein (MWt ca.
29000) initiate replication by binding to two sequences of 19-bp
DIRECT REPEATS (ITERONS), designated incB and incC, located
either side of the E-encoding gene (close to the origin of
replication); the bound molecules of E protein contribute to a
nucleoprotein complex which is a pre-requisite for replication.
Control of replication (and, hence, of COPY NUMBER) is achieved
by controlling the intracellular level of E protein to that
295
F plasmid
F430 See METHANOGENESIS.
Fab portion (Fab fragment) Either of two identical portions of
an IMMUNOGLOBULIN monomer which can be released by certain
enzymes (e.g. PAPAIN); the remainder of the molecule is termed
the Fc portion (q.v.). Each Fab portion consists of a light chain
linked via a disulphide bond to the N-terminal part of a heavy
chain, i.e., it is one of the two limbs of the Y-shaped Ig molecule.
Each Fab portion of an antibody contains a single COMBINING SITE
and behaves as a non-precipitating univalent antibody. Under
acid conditions, MERCAPTOETHANOL splits the Fab portion into
the heavy chain segment (the Fd portion) and the light chain.
F(ab )2 portion Part of an IMMUNOGLOBULIN monomer released
by the proteolytic action of PEPSIN (which also degrades at
least part of the remainder of the Ig molecule); it includes
both FAB PORTIONS connected by the HINGE REGION. The F(ab )2
portion of an antibody behaves as a bivalent, precipitating, noncomplement-fixing antibody.
facial eczema (vet.) See SPORIDESMINS.
facilitated diffusion An energy-independent TRANSPORT SYSTEM
in which the diffusion of a substance across a membrane
is facilitated by a membrane-bound protein carrier system;
in facilitated diffusion a substance necessarily passes down
a concentration gradient. Unlike simple diffusion, facilitated
diffusion exhibits MichaelisMenten saturation kinetics, it is
relatively substrate-specific, and it is subject to competitive
inhibition the uptake of one substance being inhibited by
the presence of another, structurally similar, substance. In
e.g. Saccharomyces cerevisiae various sugars, amino acids and
vitamins can be taken up by facilitated diffusion although,
depending on conditions, the same substances may also (or
alternatively) be taken up by other transport mechanisms. In
Escherichia coli, glycerol can cross the cytoplasmic membrane
by facilitated diffusion, the membrane containing a specific
facilitator protein (see also MIP CHANNEL); once inside the cell
the glycerol is phosphorylated.
FACS Fluorescence-activated cell sorter: an instrument used for
analysing and/or sorting cell populations by FLOW MICROFLUOROMETRY. Essentially, the cells (in suspension) move down a
thin, open-ended tube and, in doing so, each cell passes momentarily through a laser beam which crosses the liquid column at
right angles. As each cell passes through the beam it gives rise
to a scatter signal (scattered laser light), and also if labelled
with a FLUOROCHROME (e.g. TEXAS RED) a FLUORESCENCE signal. By using antibody-conjugated fluorochromes it is possible
e.g. to determine the presence or number of homologous antigens or receptor sites on the cell surface, since the strength
of the fluorescence signal is proportional to the amount of fluorochrome bound to the cell surface. In the dual parameter
mode, cells may be pre-treated, simultaneously, with antibodies
of two different specificities each being conjugated with a different fluorochrome; each cell passes through two separate laser
beams (of wavelengths dependent on the fluorochromes chosen)
and the two fluorescence signals are interpreted separately.
The FACS can also be used e.g. to monitor the proportion of
proliferating lymphocytes in a population, measurement being
based on the increased content of DNA in proliferating cells;
cells are initially permeated with an agent (e.g. mithramycin)
which can interact with intracellular DNA to form a complex
which fluoresces on irradiation.
Cell sorting involves the physical separation of cells into
subpopulations. Essentially, ultrasonic energy is applied to the
nozzle through which the stream of liquid (i.e. cell suspension)
passes, thus breaking up the stream into a series of very
Faulschlamm
feedlot bloat See BLOAT.
Feekes scale (plant pathol.) A scale of numbers which indicate
the various growth stages of wheat and barley: 15, shoot emergence and tillering; 610, stem elongation; 10.110.5, heading
(ear development); 11.111.4, grain ripening. Feekes scale does
not allow as detailed a designation of plant development as does
ZADOKS CODE, and is limited to wheat and barley.
felid herpesvirus 1 Syn. FELINE RHINOTRACHEITIS virus.
feline AIDS See FELINE LEUKAEMIA VIRUS.
feline calicivirus (FCV; cat flu virus; feline rhinotracheitis virus;
feline picornavirus) A virus (family CALICIVIRIDAE) which
infects the respiratory tract (occasionally also the gastrointestinal
tract) of cats, causing e.g. rhinitis, conjunctivitis, oral ulceration,
and pneumonia; the disease ranges from mild to fatal. An
attenuated strain of FCV is used as a vaccine. FCV can be
propagated in feline cell cultures. (cf. FELINE RHINOTRACHEITIS.)
feline coronavirus See CORONAVIRIDAE.
feline immunodeficiency virus (FIV) A retrovirus of the subfamily LENTIVIRINAE, originally isolated as a T-lymphotropic
virus from domestic cats with an immunodeficiency-like syndrome [Science (1987) 235 790793]; the virus can give rise
to illness resembling AIDS in humans and FAIDS (see FELINE
LEUKAEMIA VIRUS) in cats.
The FIV virion, 120150 nm in size, contains a characteristic lentivirus-type nucleocapsid. The genome 9.5 kb contains some open reading frames (as well as gag, pol and env
regions) within terminal LTRs; the ORFs apparently encode regulatory function(s).
Horizontal transmission is believed to occur typically as a
result of fighting and biting (cf. FeLV). Vertical transmission
by asymptomatic, chronically infected mothers has not been
reported, but the virus can be transmitted via milk following
experimental infection.
[Haematological disorders associated with feline retrovirus
infections (FeLV and FIV): BCH (1995) 8 73112.]
feline infectious peritonitis virus See CORONAVIRIDAE.
feline leukaemia virus (FeLV) A retrovirus (subfamily ONCOVIRINAE, type C), strains of which cause important diseases in cats;
there are many exogenous and some endogenous strains of the
virus.
The FeLV virion is roughly spherical and is 110120 nm
in diameter. The proviral DNA (of replication-competent
strains) approximately 8.4 kb in length includes the usual
retroviral gag, pol and env regions between 5 and 3 LTRs; the
expression of proviral genes is under the regulation of cis- acting promoter and enhancer regions located in the U3 sequence
of the LTR.
FeLV is transmitted horizontally, apparently via the oronasal
route, by repeated social contact; transmission also occurs
vertically, by intrauterine infection of the developing embryo.
Animals which develop chronic viraemia are sources of hightitre infectious FeLV virions (which occur in plasma and in nasal
secretions and saliva).
In over one half of the cats exposed to FeLV, the humoral and
cell-mediated defence systems succeed in abolishing detectable
virus in plasma. Nevertheless, in at least a proportion of
animals the virus can remain latent for a period of time in
myelomonocytic precursors in the bone marrow and in stromal
fibroblasts; however, it is thought that spontaneous reactivation
of latent virus in nature occurs only rarely.
FeLV causes neoplastic, degenerative and immunosuppressive
forms of disease, the latter including a syndrome resembling
human HIV-AIDS (feline AIDS or FAIDS ); other conditions
fentin
include myeloid leukaemias, anaemia, marrow aplasia, and
lymphosarcomas. (A FAIDS-like syndrome can also be caused
by the FELINE IMMUNODEFICIENCY VIRUS.)
Typically, chronic infection with FeLV involves a gradual
decrease in the numbers of lymphocytes and a reduction in
the function of both T and B cells, thus leading to clinical
immunodeficiency. Certain strains of FeLV, however, cause an
acute immunodeficiency syndrome (FAIDS).
Isolates of FeLV are often replication-competent and vonc , but ONCOGENE-containing sarcoma-inducing recombinant
viruses (feline sarcoma viruses) have been isolated from FeLVassociated tumours. Several oncogenes (e.g. FES, abl, sis) have
been reported to confer on FeLV the ability to induce sarcomas.
Insertional mutagenesis by FeLV of the host cells c-myc
oncogene is found in a significant proportion of spontaneous
and experimentally induced lymphomas.
In some experimentally induced lymphomas, the location at
which the provirus integrates in the cells genome suggests that
enhancer activity associated with the proviral LTR region may
stimulate expression of c-myc and, in this way, contribute to
pathogenesis.
The exogenous, replication-competent FeLVs are divided into
subgroups A, B and C on the basis of (i) differences in
the viral envelope glycoprotein, (ii) the interference pattern in
vitro, and (iii) susceptibility of the viruses to neutralization by
specific antibodies; differences in the envelope glycoprotein are
associated with differences in the host cell range of the various
strains of FeLV.
Subgroup A strains of FeLV are widespread and readily transmissible although apparently not highly pathogenic. Subgroup
B strains may arise through in vivo recombination and may be
more pathogenic than the A strains; in infected animals, B strains
are reported to be invariably accompanied by A strains. C strains
are said to be comparatively rare, and are associated with pure
red cell aplasia.
Various germ-line-transmissible endogenous retroviruses may
be detectable in the genome of uninfected animals. In some
cases the endogenous virus contains sequences homologous to
FeLV (enFeLV strains); in other cases (RD-114 viruses) there is
no apparent genetic relationship with FeLV. Although enFeLV
proviral DNA may not give rise to infectious virions, it may
nevertheless contribute to pathogenicity; thus, e.g. expression
of enFeLV genes has been detected in both FeLV-positive
and FeLV-negative lymphomas. Moreover, enFeLV-encoded
product(s) may represent the entity referred to as FOCMA.
Diagnosis of persistent infection by FeLV. In cells that harbour
a replication-competent strain of FeLV, viral proteins and virions
are commonly produced at a high rate. One particular protein,
the Pr65 gag precursor protein, is produced in excess and can
be easily detected in the blood of infected cats by immunoassay
techniques.
[Haematological disorders associated with feline retrovirus
infections (FeLV and feline immunodeficiency virus): BCH
(1995) 8 73112.]
feline panleukopenia virus (FPV) A subspecies of feline parvovirus (genus PARVOVIRUS). Like CANINE PARVOVIRUS (CPV),
the ssDNA genome (5100 nt) encodes two structural proteins (VP1, VP2: the mRNAs transcribed from overlapping
sequences) and two non-structural proteins. DNA from FPV and
CPV isolates is almost identical; the host range of these viruses
depends on small differences in the composition of the capsid: less than 10 amino acids determine whether a given virus
can relicate in dogs or cats. The virion retains infectivity for
days/weeks in the environment.
FepA protein
fermenter (fermentor) A vessel in which an aerobic or anaerobic
FERMENTATION (sense 2) can be carried out either in BATCH CULTURE or in CONTINUOUS CULTURE. (cf. BIOREACTOR.) Fermenters
are typically vertical, essentially closed, cylindrical steel vessels.
The traditional STIRRED TANK REACTOR is a squat vessel, but other
types are column (= tower) fermenters in which the vessel
(the column) has a height-to-diameter ratio of up to ca. 10
(e.g. the typical AIRLIFT FERMENTER, BUBBLE COLUMN FERMENTER,
JET LOOP FERMENTER, and PROPELLER FERMENTER). Important features of fermenter design include provision for: (i) Adequate
heat transfer from the culture. (The heat produced from a given
substrate can be estimated from the value of 110 kcal/mole O2
taken up a value obtained empirically using various substrates
and organisms [Book ref. 11, p. 32].) (ii) Efficient mixing of the
culture. (iii) Efficient oxygen-to-liquid transfer. (iv) Adaptability
to a range of operating conditions. (v) Ease of scale-up from the
laboratory or pilot stage to industrial use. These factors largely
determine the economics of a fermentation and the type of fermenter required for a particular purpose; thus, e.g., an STR but
not a bubble column or airlift fermenter would generally be
considered suitable for the fermentation of a (viscous) mycelial
culture since only the STR (which has a greater input energy)
would be able to ensure adequate mixing.
FernandezMoran particles The stalked particles (the F1 parts
of (F0 F1 )-type PROTON ATPASES) on the inner surface of the
mitochondrial inner membrane.
Fernandez reaction See LEPROMIN TEST.
ferredoxins A category of simple IRONSULPHUR PROTEINS which
are involved only in electron transfer processes; a given ferredoxin may contain one or more ironsulphur centres of the
type [2Fe2S], [3Fe3S] and/or [4Fe4S]. Ferredoxins typically have low-potential (i.e., highly negative) Em values; thus,
e.g. a [4Fe4S] ferredoxin (Fd I) in Desulfovibrio gigas has an
Em of 455 mV, and a (2[4Fe4S]) ferredoxin in Clostridium
pasteurianum has an Em of 400 mV. However, a [2Fe2S]
ferredoxin in Pseudomonas putida (putidaredoxin) has an Em of
240 mV. (See also HIPIP; cf. FLAVODOXINS.)
ferrichrome See SIDEROPHORES.
ferrimycins See SIDEROMYCINS.
ferrioxamines See SIDEROPHORES.
ferritin An iron-storage protein which occurs e.g. within various
mammalian, plant and fungal cells; iron is stored within the
large, hollow ferritin molecule. (cf. SIDEROPHILINS; see also
IMMUNOELECTRON MICROSCOPY.)
ferrocene monocarboxylic acid See BIOFUEL CELL.
ferrochelatase See HAEM.
ferruginous Rust-coloured.
fertility factor Syn. F PLASMID.
fertility inhibition (of the F plasmid) Inhibition of expression of
the traJ gene (and, hence, inhibition of the TRANSFER OPERON)
FERMENTATION (diagrammatic): the fermentation of an organic substrate showing intermediates undergoing mutual oxidation and reduction.
300
Fijivirus
by the intracellular presence of an IncF plasmid which encodes
a functional finO product (see FINOP SYSTEM); a plasmid which
encodes such a finO product is designated fi+ (fertility inhibition
positive) or fin+ . Compatible plasmids which do not encode a
functional finO product are designated fi .
ferulate 3-Methoxy-4-hydroxycinnamate.
Fervidobacterium See BACTERIA (taxonomy).
fes
An ONCOGENE present in the SnyderTheilen and GardnerArnstein strains of feline sarcoma virus (see FELINE
LEUKAEMIA VIRUS); v-fes is closely related to v-fps (present in
Fujinami AVIAN SARCOMA VIRUS) and may be derived from a
related c-onc sequence. The products of v-fes and v-fps have
tyrosine-specific protein kinase activity.
FeS protein (Fe/S protein) See IRONSULPHUR PROTEINS.
fescue foot (fescue toxicity syndrome) A condition which affects
animals (mainly cattle) grazing pastures dominated by tall fescue
grass (Festuca arundinacea); symptoms: lameness, followed by
dry gangrene of the extremities (tail tip, hooves, ears). It appears
to be caused by a vasoconstrictive mycotoxin produced by fungi
parasitic or pathogenic in the grasses; fungi which have been
implicated include Aspergillus terreus and biotypes of Epichloe
typhina [AEM (1977) 34 576581].
Festuca necrosis virus See CLOSTEROVIRUSES.
Feulgen reaction A specific staining reaction for DNA in situ.
Mild acid hydrolysis of DNA (e.g. with 1 N HCl) removes
purine bases and makes available the aldehyde group of the
deoxyribose; aldehyde groups react with SCHIFFS REAGENT to
give a purple coloration.
fever blister Syn. COLD SORE.
Ff phages F-specific filamentous phages (e.g. fd, f1, M13, ZJ/2):
see INOVIRUS.
ff. sp. See FORMA SPECIALIS.
Ffh See PROTEIN SECRETION.
FH4 TetrahydroFOLIC ACID.
FHA See WHOOPING COUGH.
FhuA protein Syn. TONA PROTEIN.
fhuBfhuD genes See SIDEROPHORES.
FhuE See IRON.
fi plasmid See FERTILITY INHIBITION.
fi+ plasmid See FERTILITY INHIBITION.
FIAC (2 -deoxy-2 -fluoro-5-iodo-1-b-D-arabinosylcytosine) An
ARABINOSYL NUCLEOSIDE which has antiviral activity against
herpes simplex viruses 1 and 2, varicella-zoster virus and
cytomegaloviruses in cell cultures; its mode of action resembles that of ACYCLOVIR. In trials, FIAC gave better control of
progressive herpes zoster than did vidarabine; it can be administered orally.
fibrillae See FIMBRIAE.
fibrillum See FIMBRIAE.
fibrin A fibrous, insoluble protein present e.g. in blood clots;
during normal blood-clotting, fibrin is formed from the plasma
protein FIBRINOGEN by the action of thrombin in the presence of
Ca2+ . (See also COAGULASE.)
fibrinogen The soluble glycoprotein precursor of FIBRIN. It consists of two identical monomers each comprising three chains
designated a, b and g; the chains and monomers are held together
by disulphide bridges. [Review of fibrin and fibrinogen: ARB
(1984) 53 195229.]
fibrinolysin (plasmin) An enzyme which, in mammals, is responsible for dissolving blood clots by the proteolytic degradation of
fibrin. Fibrinolysin is formed from an inactive precursor (profibrinolysin, plasminogen) normally present in the blood. The term
fibrinolysin has also been applied to various microbial enzymes
capable of direct or indirect FIBRINOLYSIS.
ILLUMINATION.
field diaphragm (in MICROSCOPY) (1) See KOHLER
(2) (Syn. field stop) A metal annulus attached to the inside of an
eyepiece at the focal plane of the eyepiece lens.
field mushroom See AGARICUS.
Fields stain A water-based staining procedure for detecting e.g.
Plasmodium spp and trypanosomes in thick blood smears. The
smear is immersed in a solution of azure, rinsed, immersed in
a solution of eosin, rinsed, and allowed to dry in air; the water
used for staining and rinsing should have a pH of 7.07.2. Any
parasites present will not be obscured by erythrocytes since the
latter are lysed during the procedure; lysis occurs because a
methanol fixation stage is omitted.
fi`evre boutonneuse Syn. BOUTONNEUSE.
fifth disease Syn. ERYTHEMA INFECTIOSUM.
figwort mosaic virus See CAULIMOVIRUSES.
Fiji disease A SUGARCANE DISEASE, caused by a FIJIVIRUS and
transmitted by planthoppers (Perkinsiella spp), which is characterized by stunting and the formation of GALLS on the underside
of leaves. Pseudo-Fiji diseases of sugarcane include one similar
to MAIZE WALLABY EAR DISEASE.
Fijivirus (plant reovirus subgroup 2) A genus of plant viruses of
the REOVIRIDAE. Genome: 10 dsRNA molecules. Members infect
plants of the Gramineae, and some can cause important diseases
of crop plants; symptoms typically include stunting, excessive
tillering, enations, and unnaturally dark-green leaves. Transmission occurs propagatively via plant-hoppers (Perkinsiella spp) in
which transovarial transmission may occur. Type member: Fiji
disease virus. Three serotypes of fijiviruses are recognized (host
and geographical range in parentheses):
Group I: cereal tillering disease virus (CTDV) (barley, oats,
maize, wheat; Sweden); maize rough dwarf virus (MRDV)
301
filament
terminal sessile basidiospores; blastospores may be formed,
teliospores are not. Members have a yeast-like vegetative phase,
with globose, oval, apiculate or elongate cells which reproduce
by budding. Conjugation between two haploid cells is followed
by the formation of a dikaryotic mycelium on which the basidia
develop. Most strains are heterothallic. The family includes the
genera CHIONOSPHAERA, FILOBASIDIELLA, and FILOBASIDIUM. (See
also WALLEMIA.)
The taxonomic position of the family is unsettled. It has
been included e.g. in the Ustilaginales, and in a separate
order (Filobasidiales) [discussion and refs: Book ref. 100, pp.
468469]; some authors [Book ref. 64] include the above three
genera in the SPORIDIALES.
Filobasidiella
A genus of fungi (see FILOBASIDIACEAE). The
yeast-like vegetative cells have CAPSULES, the size of the capsule
depending on environmental conditions. The dikaryotic hyphae
have clamp connections and dolipore septa which lack parenthesomes. Basidiospores are formed in long chains by basipetal
budding from 4 sites on the apex of the basidium. The sole
species, F. neoformans, has two varieties F. neoformans var.
neoformans (anamorph: Cryptococcus neoformans var. neoformans) and F. neoformans var. bacillispora (anamorph: Cryptococcus neoformans var. gattii ) and four serotypes (AD).
Strains have been isolated from pigeon excreta, soil, and humans
(see CRYPTOCOCCOSIS). [Book ref. 100, pp. 472482.]
Filobasidium
A genus of fungi (see FILOBASIDIACEAE). The
dikaryotic hyphae have clamp connections and dolipore septa
with or without parenthesomes. Basidia are produced laterally
and terminally on the hyphae, and sessile basidiospores are produced on a whorl at the apex of the metabasidium. Species:
F. capsuligenum (anamorph: Candida japonica), isolated e.g.
from cider and sake; F. floriforme (anamorph: possibly Cryptococcus albidus var. albidus on the basis of physiological characteristics), isolated from plants; and F. uniguttulatum (anamorph:
Cryptococcus uniguttulatus), isolated from clinical specimens.
[Book ref. 100, pp. 483491.]
filoplasmodium See LABYRINTHULAS.
filopodium See PSEUDOPODIUM.
filose Thread-like.
Filosea A class of amoebae (superclass RHIZOPODA) which form
long, tapering, hyaline filopodia that often branch and sometimes
anastomose, and that are used for trapping prey. Spores and flagellated stages are not formed. Orders: Aconchulinida (cell naked,
i.e., non-testate: e.g. NUCLEARIA, Vampyrella) and Gromiida (cell
enclosed by a siliceous or proteinaceous and membrane-like test:
e.g. EUGLYPHA, Gromia).
Filoviridae A family of viruses originally proposed to accomodate Marburg virus and Ebola virus [Intervirol. (1982) 18
2432], causal agents of clinically similar VIRAL HAEMORRHAGIC
FEVERS in man (see MARBURG FEVER). The viruses occur in various parts of Africa; man is presumed to be infected only incidentally. Monkeys and rodents can be infected experimentally,
infection usually resulting in fatal disease.
Marburg and Ebola viruses are morphologically similar and
genetically related but serologically distinct. The virions are
pleomorphic filaments of uniform width (80 nm) but variable
in length (up to 14000 nm); the unit length (i.e. the shortest
length with maximum infectivity) is 790 nm for Marburg
virus, 970 nm for Ebola virus. Ring-shaped or branched
structures are sometimes seen.
The virion consists of a helical nucleocapsid surrounded by
an envelope bearing surface spikes. [Ebola virus proteins: Virol.
(1985) 147 169176]. The genome is one molecule of negativesense ssRNA. Virions are stable at room temperature but can
fim operon
be inactivated by heat (e.g. 60 C/30 min), ultraviolet radiation
and gamma radiation, organic solvents, phenolic disinfectants,
hypochlorite and b-propiolactone.
Virus replication occurs in the host cells cytoplasm; maturation involves budding of preformed nucleocapsids through the
plasma membrane.
Marburg and Ebola viruses can be grown in various types of
cell culture (e.g. Vero cells). Infected cells exhibit CPEs such
as intracytoplasmic vesiculation, swelling of mitochondria and
degeneration of organelles.
[Book ref. 148, pp 11111118.]
Attempts to elicit protective immunity to Ebola virus in the
traditional way have not been successful. However, an approach
termed genetic vaccination (= genetic immunization), in which
plasmid DNA (encoding viral proteins) is injected into the host,
has achieved some success in an animal model: when vaccinated
in this way, guinea pigs were protected against a lethal challenge
of Ebola virus, protection correlating with both antibody titre and
the antibody-specific T cell response [Nature Medicine (1998) 4
3742]. (See also DNA VACCINES.)
The Ebola virus glycoprotein is reported to be the main viral
determinant of vascular cell cytotoxicity and damage [Nature
Medicine (2000) 6 886889]. The synthesis of increased
amounts of glycoprotein by a mutant virus was associated with
a higher level of cytotoxicity [Science (2001) 291 19651969].
A combination of DNA immunization and boosting with an
adenoviral vector (encoding relevant antigenic proteins) has been
successful in generating protective immunity against the Ebola
virus in non-human primates (cynomolgus macaques) [Nature
(2000) 408 605609].
[Asymptomatic Ebola infection (in contacts of symptomatic
patients): Lancet (2000) 355 22102215. On the trail of Ebola
and Marburg viruses: Science (2000) 290 923925.]
filter-paper cellulose See FP-CELLULOSE.
filterable virus An obsolete term originally applied to any infectious agent which could pass through the early microbiological
filters (e.g. the Berkefeld candle). Such agents included viruses
but also e.g. Chlamydia and mycoplasmas.
filtration Filtration can be used to separate microorganisms from
a liquid or gas in which they are dispersed; it is used e.g.
for the following purposes. (a) The sterilization of e.g. heatlabile liquids (known to be free of small viruses or viroids)
by passing them through a filter capable of retaining all
other microorganisms. (b) The preparation of cell-free culture
filtrates for the recovery of extracellular enzymes, antibiotics
etc. (c) The counting of small numbers of bacteria in a large
volume of liquid used e.g. in water bacteriology. A measured
volume of the sample is passed through a membrane filter
(pore size e.g. 0.45 m see below) and the membrane is
subsequently incubated, face upward, on a pad of absorbent
material which has been saturated with a suitable liquid culture
medium. The number of bacteria per unit volume is calculated
from the number of colonies which develop on the membrane.
Membranes overprinted with a grid facilitate colony counting.
(See also DEFT and COUNTING METHODS.) (d) Estimation of
particle size in a monodisperse system. The suspension is filtered
through a series of membranes of progressively smaller pore
size; assuming minimal adsorption, particle size corresponds
approximately to the pore size of the first membrane to effect
significant retention of the particles. (See also sand filter in
WATER SUPPLIES.)
Many different types of filtering apparatus have been devised.
In the majority of these, liquid is drawn through the filter
fimbriae
Classification of fimbriae. The different types of fimbria on
Gram-negative bacteria can be grouped into categories on the
basis of e.g. (i) homology in the amino acid sequences in major
subunit proteins; (ii) physical, antigenic and adhesive characteristics; and (iii) the mechanism of secretion and assembly.
One group comprises the type I fimbriae (also called type 1
fimbriae); these include: (i) the common type I fimbriae of
Escherichia coli, (ii) the P FIMBRIAE and (iii) the K88 and K99
fibrillae.
Another well-studied category of fimbriae, the type IV (=
type 4) fimbriae, are found on a range of pathogenic bacteria;
these fimbriae occur e.g. on strains of EPEC and ETEC, on
Neisseria spp and Pseudomonas aeruginosa, and on Vibrio
cholerae (toxin co-regulated pili (TCP) which constitute an
important virulence factor in CHOLERA).
Type I fimbriae (type 1 fimbriae; F1 fimbriae; common pili).
These fimbriae are chromosomally encoded and are common
e.g. on Escherichia coli and other enterobacteria. Each fimbria
consists primarily of the main rod-shaped region, about 7
nm in diam., which comprises several thousand copies of the
major pilin subunit, FimA (encoded by the fimA gene). The
distal end of the fimbria consists of a short (16 nm) and
narrow (23 nm diam.) flexible structure the fibrillum (plural:
fibrillae) which is composed of the minor pilin subunits FimF,
FimG and FimH; FimH is a mannose-binding ADHESIN which
appears to be the most distal pilin in the fibrillum.
Type I fimbriae can adhere to various cells and surfaces,
including guinea-pig and horse erythrocytes causing HAEMAGGLUTINATION; such adhesion is inhibited by D-mannose, or by
methyl-a-D-mannoside, i.e. binding is mannose-sensitive, and
type I fimbriae are said to cause mannose-sensitive haemagglutination (MSHA). Fimbriae whose adhesion is not inhibited in
this way are said to cause mannose-resistant haemagglutination
(MRHA).
Type I fimbriae can also bind to UROPLAKINS (see also UPEC),
such adhesion being a preliminary step in the development of
many URINARY TRACT INFECTIONS (such as CYSTITIS). Moreover,
type I fimbriae can promote the invasion of human urinary tract
epithelium [EMBO (2000) 19 28032812].
Genetics of type I fimbriae. In Escherichia coli, type I fimbriae
are encoded by the fimAfimH operon; fimA and fimFGH are
structural genes (see above), while the fimCD products are
involved in assembly (see later).
The fimBE genes have a regulatory role, being involved in
PHASE VARIATION: the on/off switching of fimbrial synthesis.
Switching involves inversion of a 314-bp sequence that contains
the promoter of the first structural gene in the operon, fimA.
When the control sequence is in one orientation the promoter is
located correctly for transcription of fimA and of the other genes
(so that fimbriae are synthesized); when the control sequence
is in the opposite orientation, fimA is promoter-less (so that
fimbriae are not synthesized) (cf. flagellar PHASE VARIATION in
Salmonella). The products of the fimBE genes are recombinases
which mediate inversion of the control sequence; FimB can bring
about inversion in either direction (i.e. it can switch synthesis
from on to off and from off to on), whereas FimE can mediate
only the on-to-off switch. (Under in vivo conditions, switching
also requires other (intracellular) factors, including INTEGRATION
HOST FACTOR and the HNS PROTEIN.)
Interestingly, there is evidence of regulatory cross-talk
between the fim operon and the pap operon (which encodes
P FIMBRIAE) this resulting in inhibition of expression of type I
fimbriae. In this cross-talk, PapB, a pap regulatory protein, is
final host
Type IV fimbriae (type 4 fimbriae). All the fimbriae placed in
this category are secreted and assembled in a similar way. These
fimbriae include important (adhesive) virulence factors in a range
of Gram-negative pathogens such as Neisseria gonorrhoeae and
N. meningitidis, Pseudomonas aeruginosa, Vibrio cholerae and
certain strains of Escherichia coli (e.g. the bundle-forming pili
of EPEC). (See also LONGUS.)
The type IV fimbriae of e.g. N. gonorrhoeae are subject
to PHASE VARIATION (on/off switching) as well as to extensive
ANTIGENIC VARIATION.
Most type IV fimbriae are encoded chromosomally (see also
PIL GENES). The bundle-forming pili of EPEC are an exception,
being encoded by a virulence plasmid (see also PATHOGENICITY
ISLAND).
Type IV fimbriae are typically flexible, rod-like appendages,
56 nm in diam. and 12 m in length; constituent pilins are
apparently organized in a helical fashion.
In a recent model for the assembly of type IV fimbriae in
N. gonorrhoeae [FEMS Reviews (2000) 24 2144 (3135)],
the assembly of these appendages (unlike the assembly of type I
fimbriae) begins at a protein complex in the cytoplasmic membrane; that is, the base of the fimbria is linked to the cytoplasmic
membrane a column of assembled subunits passing from this
origin, through the periplasm, through the outer membrane (see
later), and into the extracellular environment.
The adhesive properties of type IV fimbriae are due, at least
partly, to the major (structural) pilins in contrast to type I
fimbriae, in which there are minor pilins specialized for adhesion
in the distal fibrillum. Exceptionally, tip adhesins (encoded
by the pilC gene) have been indentified in the two major
pathogenic species of Neisseria [Nature (1995) 373 357359;
Mol. Microbiol. (1997) 23 879892].
Secretion and assembly of type IV fimbriae. In the model for
assembly of type IV fimbriae in N. gonorrhoeae, the major pilin
subunit, PilE, is translocated across the cytoplasmic membrane
but initially remains attached to the membrane by an N-terminal
hydrophobic sequence; this sequence is subsequently cleaved, so
that the PilE subunits can be incorporated, sequentially, into the
nascent fimbria incorporation being mediated by a complex
of proteins (including PilFGT) located within the cytoplasmic
membrane. A SECRETIN, PilQ, forms a pore (5.5 nm diam.)
in the outer membrane through which the developing fimbria
extends to the exterior; the pore is stabilized by PilP. In
N. gonorrhoeae (and N. meningitidis), the distal end of the
fimbria has an adhesive subunit, PilC (which is synthesized with
a sec-dependent signal sequence); the incorporation of PilC is
one of the initial steps in the assembly process.
[Type IV fimbriae (review): ARM (1993) 47 565596.]
PSA fimbriae (PSA pili) occur as a polar tuft in many strains
of Pseudomonas aeruginosa; they are apparently chromosomally
encoded, retractable filaments, ca. 6 nm in diam. and <1 to
several micrometres in length. PSA fimbriae act as receptors for
a range of bacteriophages.
[Secretion and assembly of regular surface structures (fimbriae, flagella and S layers) in Gram-negative bacteria: FEMS
Reviews (2000) 24 2144.]
fimbriate (1) Having FIMBRIAE. (2) Having a fringed edge.
fimbrillin See FIMBRIAE.
fimbrin See ACTIN.
fin+ plasmid See FERTILITY INHIBITION.
fin rot See BACTERIAL FIN ROT.
final host (definitive host) In heteroxenous coccidia: the host in
which the sexual phase occurs (see EIMERIORINA).
finger-and-toe disease
finger-and-toe disease See CLUBROOT.
finger millet mosaic virus See RHABDOVIRIDAE.
fingerprinting Any procedure which gives a strain-specific pattern of products when a given organism is examined; the
products commonly consist of fragments of DNA (or RNA)
distributed electrophoretically in a gel. A fingerprint may be
generated e.g. by restriction of chromosomes followed by ELECTROPHORESIS of the products (see e.g. DNA FINGERPRINTING) or
by electrophoresis of the products formed in TYPING procedures
that involve nucleic acid amplification (e.g. AFLP).
FinkelBiskisJinkins murine sarcoma virus See FBJ OSTEOSARCOMA VIRUS.
FinOP system In most IncF plasmids: a system in which
the plasmids finO and finP products act, jointly, to inhibit
translation of the traJ gene (the gene which exerts a positive
regulatory influence on the transfer genes); as a consequence of
this activity, the transfer function of such plasmids is repressed.
The FinO products of most IncF plasmids are interchangeable
but the FinP products of different plasmids are commonly not
interchangeable. [Nucleotide sequences of finP alleles of five
IncF plasmids: JB (1986) 167 754757.]
The finP product is an antisense RNA molecule which
binds to the 5 end of traJ mRNA (including the ribosomebinding sequence), thus inhibiting translation; the finO product (a polypeptide) binds to, and promotes the stability of, the
FinPmRNA duplex resulting in repression of the traJ gene
and (therefore) repression of transfer (so-called fertility inhibition). (The FinOP binding site was formerly designated fisO, OJ
or traO.)
Mutant (defective) finO and/or finP products may fail to
inhibit the expression of traJ in which case the negative
regulation of the transfer genes is abolished, and the transfer
function is expressed constitutively. Plasmids containing mutant
finO genes include R1drd 19 and R100-1.
It was originally thought that the (constitutively derepressed)
F PLASMID lacked a finO locus [Book ref. 161, p 605]. finO is
now known to be present but is inactivated by an INSERTION
SEQUENCE (IS3 ) located within the coding region of the gene.
(See also FERTILITY INHIBITION.)
fireblight A disease which can affect many members of the
Rosaceae, e.g. apple and pear trees, cotoneaster and hawthorn;
it is characterized by wilting and by browning and necrosis of
blossoms, fruit, leaves and twigs. The causal agent, Erwinia
amylovora, infects e.g. via blossoms and/or wounds; virulent
strains of E. amylovora form AMYLOVORIN. [Review: Book
ref. 58, pp. 4563.]
firefly luciferin See BIOLUMINESCENCE. (See also CHEMILUMINESCENCE.)
Firmibacteria A proposed class of bacteria comprising all organisms of the FIRMICUTES other than the THALLOBACTERIA.
Firmicutes A proposed division of the PROCARYOTAE comprising
bacteria in which the CELL WALL is of the Gram-positive type;
classes: FIRMIBACTERIA; THALLOBACTERIA.
Fis protein See CELL CYCLE (b).
Fischerella A genus of filamentous, thermophilic CYANOBACTERIA (section V) in which some of the cells in a mature trichome
divide in more than one plane, resulting in a partly multiseriate trichome with lateral uniseriate branches. Hormogonia are
formed from the ends of the trichomes or from lateral branches,
and are composed of small cylindrical cells which enlarge and
become rounded; heterocysts initially develop mainly in intercalary positions, and are mainly intercalary or lateral in mature
trichomes. Akinetes may be formed. GC%: 4249.
flagellar motility
together at one pole of the cell this propelling the cell forward
with the opposite pole leading. Within a uniform medium, such
smooth swimming is interrupted at intervals of ca. 1 second by
tumbling: a random, chaotic movement (lasting ca. 0.1 second)
resulting from a switch from CCW to clockwise (CW) in some
of the bunched flagella; when this happens the flagellar bundle
is disrupted, causing the random movement. (The timing of the
switch from CCW to CW in a given flagellum is apparently not
related to the timing of the switch in the other flagella.) Smooth
swimming is resumed when the majority of the flagella are again
rotating CCW.
The pattern of alternate smooth swimming and tumbling
results in a three-dimensional RANDOM WALK. Certain environmental stimuli can influence the pattern of motility leading to
a TAXIS (see e.g. CHEMOTAXIS).
Peritrichously flagellated bacteria generally reach speeds
of ca. 1030 m/second although peritrichously flagellated
cells of Thiovulum majus have been reported to swim at
600 m/second [Microbiology (1994) 140 31093116].
Speeds reported in monotrichously flagellated bacteria include
70 m/second (Pseudomonas aeruginosa) and 100 m/second
(Bdellovibrio). In these organisms, flagellar rotation may occur
for approximately equal periods of time in the CCW and CW
modes; during rotational reversal, conformational changes in the
filament and/or hook may bring about randomization of direction
(equivalent to tumbling in peritrichous cells) thus permitting
responses to environmental stimuli.
In amphitrichously flagellate bacteria the two flagella rotate
in opposite directions.
In bacteria of the order SPIROCHAETALES, motility is associated
with rotation of the periplasmic flagella this generating a
helical waveform in the outer membrane which enables the cells
to screw their way through the medium. Thus, CCW flagellar
rotation in Leptonema illini causes the anterior (i.e. forwardly
directed) end of the cell to assume a helical shape and the
cell to rotate clockwise about its longitudinal axis moving
forward with a screw-like action. Spirochaetes can reverse
direction and flex the latter movement perhaps being a means
of randomizing direction. The cells can swim through media
which are too viscous to permit motility of cells which rely on
external flagella. (Creeping or crawling movements have also
been recorded for spirochaetes in contact with solid surfaces.)
[Structure/motility of spirochaetes: JB (1996) 178 65396545.]
(b) (eukaryotic) The eukaryotic FLAGELLUM commonly beats
in an undulatory manner (usually in one plane, but sometimes e.g. in Euglena in a spiral) or in an oar-like manner
(as in Chlamydomonas). Undulations commonly originate at the
base of the flagellum and travel towards the tip.
The beating of a smooth flagellum generates forces which act
on the surrounding medium in the direction of the propagated
waves, so that the cell moves in the opposite direction (i.e. the
flagellum pushes the cell from behind). Conversely, if waves
travel from the tip to the base of the flagellum (as e.g. in
Trypanosoma), the cell swims with the flagellum leading.
In tinsel flagella, the mastigonemes appear to act as rigid,
passive structures which lie in the plane of the beat and generate
forces which act on the surrounding medium in a direction
opposite to that of the propagated waves; thus, a tinsel flagellum
undulating from base to tip will pull the cell from the front (as
e.g. in Ochromonas, and in zoospores of Phytophthora).
In some species the pattern of flagellar beating can be changed
e.g. in response to environmental conditions. For example, in
Trypanosoma the flagellum normally propagates waves from tip
FiteFaraco stain An acid-fast stain used for detecting Mycobacterium leprae in tissue sections; the procedure resembles
that for the ZIEHLNEELSEN STAIN but haematoxylin is used as
counterstain.
Fitz-HughCurtis syndrome See CURTISFITZ-HUGH SYNDROME.
FIV FELINE IMMUNODEFICIENCY VIRUS.
five-five-five test (5-5-5 test) A quantitative SUSPENSION TEST in
which a test organism is exposed for 5 min to each of a range
of dilutions of the test disinfectant; after neutralization of the
disinfectant, surviving bacteria are counted by subculturing to
pour plates. To be considered effective, a disinfectant must give a
minimum 5-log (105 -fold) reduction in cell numbers. Sporicidal
activity is assessed by using a suspension of endospores of
Bacillus cereus ATCC 9139 preheated at 80 C for 60 sec; an
effective sporicidal disinfectant must produce a minimum 1-log
decrease in viable spores.
five-kingdom classification See KINGDOM.
five-three-two symmetry (5-3-2 symmetry) See ICOSAHEDRAL
SYMMETRY.
fixation The process of killing cells while preserving their structure and organization in as life-like a condition as possible (cf.
CRYOFIXATION). Fixation involves the inactivation of enzymes,
particularly AUTOLYSINS; ideally, it also hardens cellular structures and renders cell components compatible with particular
stains. Most or all methods of fixation create ARTEFACTS. (a) Heat
fixation can be used for the fixation of smears of bacteria prior
to staining. The SMEAR is passed rapidly through a flame two
or three times; such heat-fixed smears are suitable e.g. for the
GRAM STAIN but are not suitable for observations on cell structure or morphology. (b) Chemical fixation. A chemical fixative
permeates cells and stabilizes their components by binding to
them or denaturing them. Some fixatives (e.g. ethanol, mercuric
chloride, picric acid) precipitate proteins and thus considerably
disturb cellular organization. Others (e.g. FORMALDEHYDE, GLUTARALDEHYDE, OSMIUM TETROXIDE, potassium dichromate) tend
to preserve proteins in situ. Osmium tetroxide and potassium
dichromate are also important lipid fixatives. For ELECTRON
MICROSCOPY osmium tetroxide and glutaraldehyde are often used
in e.g. alkaline phosphate buffer or cacodylate buffer. Glutaraldehyde may be used first to fix proteins (pre-fixation), and osmium
tetroxide used subsequently for the post-fixation of lipids. (See
also BOUINS FLUID, CARNOYS FLUID, POLYVINYL ALCOHOL FIXATIVE, SCHAUDINNS FLUID, ZENKERS FLUID.)
fixative A substance used for FIXATION.
fixed virus A strain of rabies virus attenuated by serial passage
e.g. through rabbits. (cf. FLURY VIRUS; STREET VIRUS; SEMPLE
VACCINE.)
FkpA See PROTEIN SYNTHESIS (protein folding).
fla genes In e.g. enterobacteria: genes involved in the synthesis
and function of bacterial flagella. [ARBB (1984) 13 5183.]
flabelliform (flabellate) Fan-shaped.
Flabellula See AMOEBIDA.
flacherie An economically important disease of silkworms
caused by a small RNA virus resembling a picornavirus (see
PICORNAVIRIDAE).
flagella Plural of FLAGELLUM.
flagellar motility (a) (bacterial) MOTILITY produced by the rotation of a FLAGELLUM, or the rotation of a number of flagella.
In peritrichously flagellated bacteria (such as Escherichia coli
and Salmonella typhimurium), the flagella rotate independently
of one another [Cell (1983) 32 109117]. For most (95%)
of the time, each flagellum rotates counterclockwise (CCW).
When the majority of flagella are rotating CCW they bunch
307
flagellar motor
to base, but during an avoiding reaction (PHOBIC RESPONSE) the
direction of wave propagation can be reversed. Chlamydomonas
normally swims with an oar-like breast stroke (ciliary-type
action), but in an avoiding reaction the two flagella extend
forwards and propagate waves from base to tip (flagellar-type
action).
In many species the flagellum is apparently capable of only
one type of movement; in these organisms changes in direction
may be achieved by a temporary cessation of beating, the
flagellum remaining bent during this period. [Dynamics of
eukaryotic flagellar movement: SEBS (1982) 35 289312.]
Flagellar movements appear to be regulated by the levels of
Ca2+ in the flagellum; some environmental stimuli appear to
cause changes in the permeability of the flagellar membrane
to calcium ions, and consequent changes in motility patterns.
In at least some species, levels of calcium ions within the
flagellum may be regulated by a Ca2+ -ATPase located in
the flagellar membrane. In Chlamydomonas reinhardtii the
photophobic response is apparently initiated by Ca2+ -stimulated
phosphorylation of certain axonemal proteins [JCB (1985) 101
17021712].
flagellar motor See FLAGELLUM (a).
flagellar phase variation See PHASE VARIATION.
flagellar stain See FLAGELLUM (a).
flagellate (1) (adj.) Bearing one or more flagella (see FLAGELLUM). (2) (noun) A protozoon of the MASTIGOPHORA.
flagellin The protein subunit of the filament of a bacterial FLAGELLUM. The composition of flagellin (MWt ca. 3000055000)
varies with species, and determines e.g. the shape of the flagellum, its antigenic specificity (see H ANTIGEN and PHASE VARIATION), and susceptibility to FLAGELLOTROPIC PHAGES. Typically,
flagellins are relatively rich in glutamate and aspartate but poor
in aromatic amino acids; cysteine is usually absent. Flagellins
from the alkalophile Bacillus firmus have a lower content of
basic amino acids [JGM (1983) 129 32393242]; the complex
flagella of Rhizobium spp have a higher content of hydrophobic amino acids. A flagellar filament may be dissociated into
its flagellin subunits e.g. by treatment with detergents or acid;
under appropriate conditions, and given a primer (e.g. a small
fragment of flagellum), the flagellin subunits can re-assemble
spontaneously.
flagellotropic phage Any BACTERIOPHAGE which adsorbs to a
host cell flagellum and hence is specific for flagellated host cells
(see also FLAGELLIN). Flagellotropic phages include e.g. bacteriophage c (see STYLOVIRIDAE) in enterobacteria, BACTERIOPHAGE
PBS1 (q.v.) in Bacillus subtilis, and bacteriophage 7-7-1 in Rhizobium lupini . In e.g. phage c, the tip of the phage tail bears a
fibre which appears to wrap around the flagellum, and the phage
then appears to move down to the base of the flagellum to infect
the cell.
flagellum (plural : flagella) (a) (bacterial) A thread-like appendage which (commonly) projects from the surface of the cell and
which is responsible for MOTILITY in most types of motile bacteria; such flagella may occur e.g. singly, in groups or tufts, or
distributed over the surface of the cell (see AMPHITRICHOUS, HELICOTRICHOUS, LOPHOTRICHOUS, MONOTRICHOUS and PERITRICHOUS).
By contrast, in bacteria of the SPIROCHAETALES the flagella
occur between layers of the cell envelope. This entry refers primarily to flagella which project from the cell surface although
the structural and mechanistic features of spirochaete flagella are
apparently similar.
Flagella can be detected by dark-field MICROSCOPY but not
by bright-field microscopy unless suitably stained (see e.g.
flagellum
FLAGELLUM: the origin of a flagellum in the cell envelope of Escherichia coli, Salmonella typhimurium and related Gram-negative bacteria
(diagrammatic, not drawn to scale; see entry).
(a) An earlier model.
(b) A current view based on several sources [e.g. JB (1996) 178 45824589; JMB (1996) 255 458475]. As in the earlier model, the L and
P rings are associated with the outer membrane and peptidoglycan layer, respectively. The MS ring previously regarded as two distinct
structures (the M and S rings) lies in the cytoplasmic membrane. The C ring, which includes proteins FliM and FliN (see table, text), is in
the cytoplasm; it is associated with the MS ring and is believed to rotate with the MS ring when the flagellar motor is running. The C ring is
involved in switching between counterclockwise and clockwise rotation of the flagellum in chemotaxis.
The annular region of the cytoplasmic membrane which encircles the MS ring contains the MotA and MotB proteins; this region acts as the
stator of the flagellar motor. It appears that MotA and MotB form a complex, with MotB bound to peptidoglycan, and MotA interacting with
molecules of the FliG protein (which are bound to the periphery of the MS ring); the latter interaction (details currently unknown) generates
torque and, hence, flagellar rotation.
The flagellar motor (= basal body) includes the L, P and MS rings, the axial rod (shaft) and the MotA/MotB complex. The C ring is included
by some authors; other authors include the C ring as part of an extended basal body.
The dotted line enclosed by the C ring represents a structure which has been termed the export apparatus (see entry) and which now
appears to be a form of type III PROTEIN SECRETION system.
Reproduced from Bacteria 5th edition, Figure 2.8, page 28, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
flagellum
FLAGELLUM (bacterial): some of the genes and gene products involved in the assembly of the flagellum in Escherichia
coli, Salmonella typhimurium and related species
Gene (product)
Class I genes
flhC (FlhC)
flhD (FlhD)
Class II genes
flgB (FlgB)
flgC (FlgC)
flgE (FlgE)
flgF (FlgF)
flgG (FlgG)
flgH (FlgH)
flgI (FlgI)
flgK (FlgK)
flgL (FlgL)
flgM (FlgM)
flhA (FlhA)
flhB (FlhB)
fliA (FliA)
fliD (FliD)
fliF (FliF)
fliG (FliG)
fliH (FliH)
fliI (FliI)
fliJ (FliJ)
fliK (FliK)
fliM (FliM)
fliN (FliN)
fliO (FliO)
fliP (FliP)
fliQ (FliQ)
fliR (FliR)
Rod (proximal)
Rod (proximal)
Hook
Rod (proximal)
Rod (distal)
L ring
P ring
Hook (distal end)
Hook (distal end)
Anti-sigma factor (delays FliA activity)
Export apparatus
Export apparatus
Sigma factor (s28 ) for class III genes
Filament cap
MS ring
Switch/C ring?/torque generation
Export apparatus
Export apparatus
Export apparatus/chaperone
Regulation of hook length
C ring/switch
C ring/switch
Export apparatus
Export apparatus
Export apparatus
Export apparatus
Flaviviridae
flaming Brief exposure of an object (or part of an object) to the
hottest part of a flame usually for the STERILIZATION of the
surface thus treated. Flaming is part of the ASEPTIC TECHNIQUE.
Objects such the LOOP and STRAIGHT WIRE are flamed for ca.
35 sec; somewhat shorter exposures are used for the rims of
e.g. bottles from which sterile (non-flammable!) substances are
to be poured. Flaming for very short times may be used for the
heat FIXATION of bacterial smears.
Flammulina
See AGARICALES (Tricholomataceae) and ENOKITAKE.
flash-freezing Syn. QUENCH-FREEZING.
flash pasteurization See PASTEURIZATION.
flask fungi PERITHECIUM-forming fungi.
flat-field objective lens An objective lens (see MICROSCOPY)
which can give an image in which all parts of the field are
simultaneously in focus. Flat-field objectives are denoted by the
prefix plan- or plano- (see e.g. ACHROMAT).
flat sour A can (see CANNING) which appears normal (i.e. the
ends are flat or slightly concave cf. SWELL) but whose contents
have been soured as a result of microbial growth; Bacillus
stearothermophilus is one of several common causal agents in
low-acid foods. (See also SOFT CORE HAM.)
flavacol A compound produced by Aspergillus flavus: 3-hydroxy2,5-diisobutylpyrazine.
flavin adenine dinucleotide See RIBOFLAVIN.
flavin mononucleotide See RIBOFLAVIN.
Flaviviridae (arbovirus group B) A family of enveloped ssRNAcontaining VIRUSES [Intervirol. (1985) 24 183192] formerly
regarded as a genus within the family TOGAVIRIDAE. Flaviviruses
infect a wide range of vertebrates, and many also infect invertebrates (mosquitoes or ticks) which act as VECTORS. Some flaviviruses are important pathogens of man or animals. The
family contains a single genus, Flavivirus; type species: yellow
fever virus.
The flavivirus virion is more or less spherical (ca. 4050 nm
diam.); it consists of a core (comprising a single type of
core protein, C, associated with the genome), a membranelike protein, M, which surrounds the CRNA complex, and
a lipoprotein envelope containing one type of virus-specific
glycoprotein, E, which acts as a haemagglutinin (e.g. with
chick RBCs) and is the target of neutralizing antibodies. The
genome is a single linear positive-sense ssRNA molecule
(MWt ca. 4 106 ) which is capped at the 5 end but is
apparently not polyadenylated at the 3 end. Subgenomic mRNA
is not produced; the genome-length RNA functions as the sole
messenger and contains only one long open reading frame at
least in West Nile virus [Virol. (1986) 149 1026] and in
yellow fever virus [Science (1985) 229 726733] suggesting
that viral proteins are formed by post-translational cleavage of a
polyprotein. The genes encoding structural proteins are located
at the 5 end (5 -CME. . .); several non-structural proteins are
also produced. A region at the 3 end is not translated and has the
potential for forming a stem-and-loop secondary structure [JGV
(1986) 67 11831188]. Viral RNA synthesis (which involves
the formation of both replicative intermediates and replicative
forms) apparently occurs in the perinuclear region; maturation
may involve a process of condensation rather than budding, and
appears to occur within cisternae of the endoplasmic reticulum.
Flaviviruses can replicate in various types of vertebrate cells
in culture, often causing CPE and plaque-formation; infected
cells typically exhibit extensive proliferation of the endoplasmic
reticulum. Host protein synthesis is not significantly inhibited.
Invertebrate cells may also be infected, with or without CPE.
Flavivirus
uredia on both sides of the leaf and, later, dark-coloured telia on
the stems.
flax wilt See FUSARIUM WILT.
Flectobacillus
A genus of pink-pigmented bacteria (family
SPIROSOMACEAE). The cells are typically C-shaped, 0.31.0
1.55.0 m, but spiral forms occur as do filaments up to
50 m; ring-shaped structures may be apparent due to overlap
of the ends of curved cells. Acid is formed from many
carbohydrates. GC%: 3440. Type species: F. major.
Flexibacter A genus of GLIDING BACTERIA (see CYTOPHAGALES)
which occur in aquatic habitats; some species are pathogenic
for fish (see e.g. COLD WATER DISEASE and COLUMNARIS DISEASE).
The cells are short, non-motile rods in old cultures but are
thin, thread-like and motile in young cultures; typically, they
contain pigments ranging from yellow to red. Metabolism:
chemoorganotrophic.
Flexibacteriae A class of non-photosynthetic GLIDING BACTERIA
comprising the orders CYTOPHAGALES and MYXOBACTERALES
[ARM (1981) 35 339364].
flexible pouch Syn. RETORT POUCH.
flexirubins Polyene pigments found e.g. in members of the
CYTOPHAGALES.
flexuous hyphae (receptive hyphae) Hyphae which project from
a pycnium and which function as female (receptive) structures.
(cf. TRICHOGYNE.)
flgM gene See SIGMA FACTOR.
fliA gene See SIGMA FACTOR.
flimmer See FLAGELLUM (b).
flimmergeissel flagellum See FLAGELLUM (b).
flipflop (of membrane lipids) See CYTOPLASMIC MEMBRANE.
flippase See CYTOPLASMIC MEMBRANE.
flipper A can (see CANNING) which appears normal but in which
one end flips out (i.e. becomes convex) if the can is struck (cf.
SWELL).
floSt gene See FLORFENICOL.
floc blanket clarifier See WATER SUPPLIES.
flocculation (1) (serol.) A term used with different meanings
by different authors and for different phenomena: e.g., (i) the
development of a flaky or fluffy precipitate in certain precipitin
tests; (ii) any form of precipitate; (iii) any form of agglutination,
but particularly the agglutination of bacteria by antiflagellar
antibodies.
(2) The aggregation of (initially separate) cells to form flocs.
Spontaneous flocculation occurs e.g. in certain sewage bacteria
(see e.g. ZOOGLOEA and CELLULOSE) and in strains of BREWERS
YEAST during the stationary phase of batch culture (e.g. at the end
of the fermentation stage of BREWING). Flocculation of brewers
yeast aids in the separation of the yeast cells from the fermented
wort. (Yeast cells which remain dispersed in all phases of batch
culture are called powdery yeasts.) Prior to flocculation, the
cells are presumed to remain dispersed because of their mutually
repulsive (usually negative) surface charge (see ZETA POTENTIAL);
flocculation is thought to be initiated by a change in the surface
structure of the cells, and Ca2+ appears to play a role by bridging
the negative charges on adjacent cells [review: Book ref. 108,
pp. 323335]. (cf. COAGGREGATION.)
flood plate A PLATE in which the surface has been flooded with
liquid inoculum and the excess drawn off with a sterile Pasteur
pipette. (See also LAWN PLATE.)
flor sherry, flor yeast See WINE-MAKING.
florfenicol A synthetic, broad-spectrum antibiotic which has
been used e.g. against Mycoplasma bovis in the treatment of
calf pneumonia. In vitro tests on field isolates of M. bovis
fluorescence
indicate that significant levels of resistance have developed
against florfenicol [VR (2000) 146 745747]. In Salmonella
typhimurium DT104 (an emergent multidrug-resistant pathogen),
mutation in gene f loSt can result in resistance to both florfenicol
and chloramphenicol [JCM (1999) 37 13481351].
Florida horse leech Syn. EQUINE PHYCOMYCOSIS.
floridean starch An amylopectin-like D-glucan: the main storage
carbohydrate in members of the Rhodophyta. [Book ref. 37, pp.
475478.]
floridoside 2-O-Glycerol-a-D-galactopyranoside: a glycoside
found in members of the Rhodophyta; it serves as a
reserve carbohydrate and as an osmoregulatory compound. (cf.
ISOFLORIDOSIDE.)
flotation A method for concentrating e.g. protozoan cysts in a
sample of faeces; the sample is dispersed in a concentrated
solution of e.g. ZnSO4 or NaCl such that any cysts present in
the sample float to the surface. (cf. FORMALINETHER METHOD.)
Zinc sulphate flotation. The faecal sample (ca. 1 g) is mixed
with about ten times its volume of water, centrifuged (ca.
350 g/3 min), and all the supernatant discarded. The sediment
is re-suspended in ca. 10 ml of a solution of ZnSO4 of S.G.
1.18 (made by adding water to 331 g ZnSO4 .7H2 O to give a
final volume of 1 litre) and filtered through a double layer of
wet gauze; the filtrate is centrifuged (ca. 350 g/3 min) the
centrifuge being allowed to stop naturally to avoid turbulence
within the liquid. A loopful of liquid from the surface is
transferred to a drop of iodine solution on a slide; a cover-glass
is added, and the preparation is examined under the microscope.
Salt flotation. A solution of NaCl (70100% saturated) is
often used for the concentration of coccidian cysts in faecal
samples. The sample is subjected to several cycles of centrifugation in water (each ca. 350 g/23 min), the supernatant being
discarded each time. The sediment is then dispersed in salt solution and centrifuged at ca. 200 g/5 min. The surface layer of
supernatant is transferred, by pipette, to ten times its volume of
water; this suspension is centrifuged and the sediment collected
for study. Prolonged contact with saturated salt solution causes
plasmolysis; however, oocysts generally remain viable, and they
regain their original appearance on transfer to water.
flotation form (of an amoeba) See PSEUDOPODIUM.
flow cytometry Any procedure in which individual cells in a
suspension are counted, sorted, or otherwise analysed by the use
of an apparatus in which the cells pass, individually, through
a small hole or tube; the term is commonly used to refer
specifically to those techniques in which cell populations are
analysed by detecting fluorescence or FLUOROCHROME-labelled
antigens or other structures on/in the cell (see e.g. FACS and
FLOW MICROFLUOROMETRY; cf. COULTER COUNTER).
flow microfluorometry Any procedure in which populations of
cells, or of other particles, are counted, sorted, or otherwise
analysed by passing them individually through a small hole
or tube and detecting specific fluorescence or FLUOROCHROME
labels. (See e.g. FACS; cf. FLOW CYTOMETRY.)
flowers of tan See FULIGO.
FLP gene See TWO-MICRON DNA PLASMID.
flu Syn. INFLUENZA.
flucloxacillin See PENICILLINS.
fluctuation test A test devised by Luria and Delbruck in 1943 for
investigating the mode in which bacterial populations respond
to changes in the environment. At that time two hypotheses coexisted. (i) Genetic changes occur adaptively, i.e., as a result of
environmental influences on the cells; those cells which adapt
to the environment survive and proliferate. (ii) Genetic changes
food poisoning
food poisoning
own uptake which occurs by the trigger mechanism. Effector molecules (secreted via the type III system) are translocated
into the epithelial cell where they bring about certain changes
(e.g. actin polymerization). During uptake, extrusions of the host
cell membrane (supported e.g. by actin elements) engulf the
bacterium which is thus internalized in a vacuole containing
extracellular fluid. Unlike Shigella (see DYSENTERY), Salmonella
invades via the apical (lumen-facing) surface of gut epithelial cells.
Salmonella multiplies within the vacuole.
Although much is now known about the way in which
salmonellae invade the epithelium, less is known about the
mechanism(s) by which infection induces intestinal secretion.
Two mechanisms have been considered: (i) the action of toxin(s),
and (ii) the effect of invasion per se. S. typhimurium is known
to produce at least one toxin: Stn, a 25 kDa protein, encoded by
gene stn, which is predicted to function as an ADP-ribosylating
agent; however, only low levels of this toxin are formed, and its
significance in pathogenesis is uncertain. It has been suggested
that invasion may stimulate certain host cell secretory pathways,
although invasion and secretion are not always correlated. (In a
veterinary context, the cattle pathogen Salmonella dublin has
been reported to secrete an effector protein, SopB, via a type
III secretory system encoded by the inv-spa genes; SopB is
believed to mediate enteropathogenicity by being translocated
into epithelial cells and inducing both inflammation and fluid
secretion [Mol. Microbiol. (1997) 25 903912].)
Recovery from Salmonella food poisoning commonly begins
within a few days, but a carrier state may persist. Complications
include sepsis and abscess formation in the meninges (in small
children), arteries (leading to arteritis and e.g. rupture of the
artery), bones and joints (cf. OSTEOMYELITIS).
(f) Shigella. See DYSENTERY.
(g) Staphylococcus. Staphylococcal food poisoning usually
follows ingestion of food containing one or more ENTEROTOXINS (q.v.) formed by toxigenic, coagulase-positive strains of
S. aureus. Commonly implicated are cooked foods eaten cold
(e.g. hams, poultry), and prepared foods such as sandwiches,
custards etc. The source of staphylococcal contamination is man
(typically a food-handler); the organisms derive from the nares
or skin, or from skin lesions (e.g. boils). [Detection of staphylococcal enterotoxins: RMM (1994) 5 5664.]
Incubation period: 16 hours. Onset is abrupt, with nausea,
vomiting, abdominal pain and prostration, sometimes with
diarrhoea. Symptoms may last for about 12 hours, but weakness
and malaise may persist.
Vomiting may result from stimulation, by the toxin, of neural
receptors in the upper intestinal tract this being suggested
by abolition of the emetic reflex (in monkeys) following
vagotomy and sympathectomy. The superantigenic nature of the
enterotoxins suggests that cytokines may play an important role
in generating at least some of the symptoms of staphylococcal
food poisoning.
(h) Vibrio parahaemolyticus. Gastroenteritis due to V. parahaemolyticus (see VIBRIO) is associated with the consumption of
raw or inadequately cooked seafoods (fish, shellfish etc.). Most
outbreaks occur during warm months. The pathogen may be
concentrated in the gut of filter-feeding shellfish (cf. SHELLFISH
POISONING) and may proliferate in contaminated seafoods stored
without refrigeration.
Incubation period: often 1224 hours, but may be less
than 2 hours (a shorter period typically correlating with more
severe symptoms). Gastroenteritis: diarrhoea commonly watery,
food preservation
sometimes explosive and dysenteric; other symptoms include
nausea, abdominal cramps, vomiting, fever and chills. The illness
may last 36 days.
The main diarrhoeagenic factor of the pathogen is a 23
kDa protein, TDH; TDH is the haemolysin responsible for the
KANAGAWA PHENOMENON. The binding site for this haemolysin (in
the rabbit) is probably a trisialoganglioside designated GT1b ; in
vitro studies indicate that the toxin promotes the secretion of
chloride.
V. parahaemolyticus is reported to be usually sensitive to
tetracycline, chloramphenicol, nalidixic acid and gentamicin
but resistant to a number of b-lactam antibiotics, including
ampicillin.
[V. parahaemolyticus in humans (review): RMM (1995) 6
137145.]
(i) Viruses. Strains of ROTAVIRUS are common causal agents
of viral gastroenteritis in infants; they infect the mucosa of the
jejunum and ileum, causing desquamation and villous atrophy.
Infection occurs by ingestion of faecally contaminated food
or water. Incubation period: 23 days. Onset is abrupt,
with vomiting and diarrhoea (often associated with an upper
respiratory tract infection). Recovery may occur in 23 days,
or the disease may be fatal. Infection in adults seems to be
largely asymptomatic.
The SMALL ROUND STRUCTURED VIRUSES (also called e.g.
parvo-like viruses or parvovirus-like agents) are major causes
of gastroenteritis in both children and adults; these infections
have been called e.g. epidemic vomiting disease, while outbreaks during the winter months have been designated winter vomiting disease. Immunity following infection may be
short-lived. Infection is thought to occur by consumption of faecally contaminated food (see e.g. SHELLFISH POISONING) or water.
Incubation period: 12 days. Onset is sudden, with nausea
and vomiting, sometimes with mild diarrhoea, fever, myalgia,
malaise etc.
(j) Yersinia enterocolitica is associated with gastroenteritis
mainly in children. The condition is often mild, with fever,
a watery diarrhoea, vomiting and abdominal pain, usually
resolving in 12 days. However, severe cases may involve
ileitis often in association with mesenteric lymphadenitis;
in these cases the severe abdominal pain may mimic acute
appendicitis (pseudoappendicitis).
Various foods have been implicated as vehicles for the
pathogen (e.g. meat, especially pork, and milk); large numbers of
cells of Y. enterocolitica have been reported in certain vacuumpacked meats (see DFD MEAT). The pathogen can grow at, and
below, 4 C (i.e. even under refrigeration).
Strains of the pathogen secrete a heat-stable enterotoxin
(designated Yst) apparently similar to the ST-I of ETEC in both
structure and activity; this toxin may be responsible for the
diarrhoeal symptoms.
Y. enterocolitica invades the intestinal mucosa studies in
animals indicating that initial entry occurs (as in Shigella) via the
M cells of Peyers patches. [Invasion by Y. enterocolitica: e.g.
Book ref. 218, pp 225228.] In one model, cells of the pathogen
pass through the M cells so that they gain access to the basolateral surfaces of adjacent epithelial cells on which are found
the receptors (integrins) of several bacterial adhesins. Adhesins
of Y. enterocolitica include the outer membrane protein invasin
(chromosomally encoded by the inv gene), and the YadA protein
(encoded by plasmid pYV) which forms a cell-surface fibrillar
matrix. Invasion via the basolateral surfaces of epithelial cells
is likely to resemble the process seen in vitro. In vitro, the
food spoilage
such structure(s) are initially enclosed within membranous
vesicles to form food vacuoles.
food yeast See SINGLE-CELL PROTEIN.
foolish seedling disease Syn. BAKANAE DISEASE.
foot (mycol.) In fungi of the Laboulbeniales: a dark, basal cell
which anchors the thallus to the host organism. (cf. FOOT CELL.)
foot and mouth disease (aphthous fever) An acute, highly infectious disease which can affect all cloven-hoofed animals e.g.
cattle, goats, pigs, sheep and e.g. hedgehogs and rodents;
horses are immune, and man is affected only rarely. The causal
agent is an APHTHOVIRUS. Infection may occur by ingestion of
contaminated food or inhalation of virus-bearing aerosols; the
incubation period is usually several days to a week, but may be
up to ca. 20 days. Symptoms include fever and the formation
of vesicles (fluid-filled blister-like lesions) on the mucous membranes of the mouth and on the feet particularly where the
horny material and skin are contiguous; the copious saliva contains viruses derived from the ruptured vesicles. Vesicles may
also appear on the teats, and viruses may also be found in the
milk, blood, urine and faeces. In adult animals the disease is
usually not fatal; however, it causes serious economic losses in
terms of meat and milk production. Control : in countries where
outbreaks occur only sporadically, control may be effected by
slaughter of infected and suspect animals; vaccination has been
used in some cases. [Protection of cattle using a synthetic peptide
vaccine: Science (1986) 232 639641.] A carrier state occurs
in cattle, goats and sheep (but not pigs). Disinfection. The virus
may persist for months in infected premises, stability being promoted e.g. by low temperatures. The virus may be destroyed
e.g. by extremes of pH citric acid solution or a 1% solution
of sodium hydroxide (caustic soda) being effective disinfectants.
Other disinfectants which have been used include iodophors (see
IODINE) and hypochlorites; phenolics are apparently effective
only if used in concentrated solutions (e.g. 1:6, 1:8). Laboratory diagnosis: e.g. culture of the virus (from pharyngeal swabs
etc) and/or a CFT.
In February, 2001, the first cases of a major outbreak of
foot and mouth disease were confirmed in the United Kingdom;
during the period FebruaryMay the number of reported cases
was particularly high in Cumbria, Dumfries and Galloway,
County Durham and Devon. (A flare-up in Northumberland
occurred in late August.) [Epidemiology (diagram of links
between confirmed cases as at March 14th, 2001): VR (2001)
148 322325.] Government policy involved timely slaughter of
both infected and suspect animals, including those on adjacent
farms (the contiguous cull). Large numbers of carcases were
burnt or buried, but burial was considered inappropriate for
cattle over a certain age owing to the presumed risk of
environmental contamination with prions of BOVINE SPONGIFORM
ENCEPHALOPATHY.
Despite the availability of vaccines, vaccination was resisted;
an important factor in this decision was the desire to maintain
the UKs disease-free status (thus protecting the export trade).
In this outbreak, some veterinary inspections revealed lesions
of unknown aetiology which could complicate the diagnosis of
foot and mouth disease [photographs of oral lesions in sheep
and cattle in Dumfries and Galloway that could complicate the
diagnosis of foot and mouth disease: VR (2001) 148 720723].
Currently, work is ongoing to improve the performance of
ELISA-based serological tests that distinguish between (i) antibodies to whole virus particles (such as those in inactivated
vaccines), and (ii) antibodies to viral proteins exposed only during replication of the virus; tests that could (reliably) distinguish
Foraminiferida
between infected, vaccinated and carrier animals could lead
to the possibility of vaccination compatible with disease-free
status [see Nature (2001) 410 1012].
In man, the disease involves fever, malaise, and the formation
of vesicles in the mouth and on the lips, hands and feet; infection
may occur via wounds or by ingestion of contaminated dairy
products. Complete recovery usually occurs. (cf. HAND, FOOT
AND MOUTH DISEASE.)
(See also SWINE VESICULAR DISEASE; VESICULAR EXANTHEMA;
VESICULAR STOMATITIS.)
foot cell (1) (mycol.) A foot-shaped terminal cell in a macroconidium of FUSARIUM. (2) (mycol.) A hyphal cell which gives rise
to a conidiophore. (cf. FOOT.)
foot-rot (foot rot; footrot) (1) (vet.) In cattle and sheep: a disease
involving infection and inflammation of the skinhorn junction
and adjacent sensitive areas of the foot, frequently resulting
in severe lameness; in sheep the causal agent is Bacteroides
nodosus (cf. SCALD), while in cattle the condition may be caused
by Fusobacterium necrophorum and/or Bacteroides (or other)
species. Foot-rot occurs typically in warm, wet weather. (Some
breeds are more susceptible than others. Bos taurus cattle appear
to be much more susceptible than Bos indicus (Zebu-type,
Brahman) breeds, and the Australasian Merino sheep tend to
be more susceptible than British breeds.) Symptoms: the foot
is tender and inflamed and has a characteristic necrotic odour,
but pus is generally not formed in large amounts. Fever may
be present. Treatment: parenteral administration of antibiotics
and/or topical application (to the cleaned, prepared foot) of e.g.
a 5% w/v CuSO4 solution; foot-baths of e.g. 5% CuSO4 , 5%
formalin, or 10% ZnSO4 are useful for control.
In pigs, foot-rot is not unlike that found in cattle and sheep, but
the condition appears to be more obviously linked to mechanical
damage to the feet, and the causal agent(s) appear to include a
wider range of species (e.g. F. necrophorum, staphylococci); a
dietary deficiency of biotin predisposes towards foot lesions in
the pig. Topical treatment and foot-baths can be effective.
(2) (plant pathol.) Any of various plant diseases in which
the base of the stem rots as a result of microbial infection;
causal agents include species of e.g. FUSARIUM, Pythium, Rhizoctonia, Sclerotium, Thielaviopsis, etc. These fungi commonly
soften the stem tissue by producing pectinolytic and possibly cellulolytic enzymes, causing the plant to collapse. (cf.
DAMPING OFF.)
footprinting In the context of proteinDNA interactions: any of
various methods used to determine the particular sequence of
DNA to which a given protein binds; essentially, the binding
site of the protein is determined by identifying that region of the
DNA molecule in which the presence of bound protein protects
(shields) the DNA from cleavage by a nuclease (e.g. DNase I)
or by certain chemical agents.
In one approach, two sets of homologous, end-labelled DNA
fragments one set carrying the bound protein are exposed to
a particular nuclease, or a chemical agent, under conditions in
which, ideally, each fragment is cut at only one of a number
of potential cleavage sites. The result is a number of labelled
sub-fragments in a range of different sizes reflecting cleavage
at different sites in different fragments. If, in protein-bound
fragments, the presence of protein obscures one or more cleavage
sites, then no sub-fragment will terminate at such protected
site(s). Consequently, if the two sets of sub-fragments are
compared by gel electrophoresis, the absence of certain size(s)
of sub-fragment from the protein-bound set will be seen as a gap
in the gel; this gap, resulting from shielding of corresponding
cleavage site(s) by the protein, is the proteins footprint.
smaller than that in the gamont test. Variations may occur in this
generalized life cycle: e.g., in Glabratella sulcata the gametes
are exchanged directly between two gamonts in contact, rather
than being released into the sea.
Most foraminifera are marine benthic organisms, although
some (e.g. GLOBIGERINA, GLOBIGERINOIDES) are pelagic (planktonic), and a few (e.g. Nonion germanicum) occur in brackish
waters. The organisms are typically holozoic and omnivorous, feeding on bacteria, small protozoa, microalgae, etc.
[Invasive activity of Allogromia pseudopodial networks: JP
(1985) 32 912.] Photosynthetic endosymbionts occur in many
foraminifera, including most or all of the large forms (e.g.
Amphistegina) which occur often abundantly in shallow
tropical and subtropical seas; depending on species, these
endosymbionts may be dinoflagellates (e.g. Amphidinium, Symbiodinium), green algae (e.g. Chlamydomonas, Chlorella),
frustule-less diatoms (which can reconstitute their frustules
in culture), or a unicellular red alga (Porphyridium?). The
endosymbionts seem able to satisfy at least a significant proportion of the carbon and energy requirements of the protozoon,
but ingestion of prey is apparently necessary to supply adequate
levels of e.g. nitrogen and phosphorus [e.g. in Globigerinoides
sacculifer : Limn. Ocean. (1985) 30 12531267]. In Nonion germanicum chloroplasts from ingested algae appear to survive
digestion for long enough to supply the protozoon with some
photosynthate. [Symbiosis: Book ref. 129, pp. 3768; potential
symbionts in bathyal species: Science (2003) 299 861.]
Fossil foraminiferan tests occur abundantly in certain oceanic
deposits and sedimentary rocks, sometimes being a major component of thick deposits of chalk (such as the white cliffs of
Dover and Normandy). (See also COCCOLITH.) Numerous genera and species of fossil foraminifera have been documented,
the earliest dating from the late Precambrian to early Cambrian
(primitive globular tests with a single aperture). Fossil tests are
commonly ca. 0.22.0 mm in diam., but some fusulinids (Carboniferous to Permian) and nummilitids (Eocene to Oligocene)
are much larger: e.g. the discoid multiloculate tests of Nummilites gizehensis may be >120 mm. A rapid succession of
distinctive species of fossil foraminifera has occurred through
the geological ages, making them ideal markers in the biostratigraphy of sedimentary rocks e.g. for oil prospecting. [Stratigraphy
of planktonic foraminifera: Book ref. 136, pp. 11328.]
foreign body giant cell See GIANT CELL.
forespore See ENDOSPORE (sense 1 (a)).
forest yaws Syn. PIAN BOIS.
form genus (mycol.) A non-phylogenetic category, equivalent to
genus, which is distinguished on the basis of one or more (typically) morphological features. Form species within a form genus
are referred to by Latin binomials (see NOMENCLATURE). (The
prefix form although taxonomically correct is frequently
omitted.)
In the DEUTEROMYCOTINA, form genera are used to classify
e.g. those fungi which have no known sexual stage; such form
genera are based primarily on the characteristics (including mode
of development) of the conidia. If the sexual stage of a form
species is discovered, the name of the form species based on
the anamorph can continue to be used, but the taxonomically
valid name is that of the teleomorph.
Form genera are also used for certain members of the
Aphyllophorales: see e.g. FOMES, POLYPORUS and PORIA.
form species See FORM GENUS.
forma specialis
(special form; f. sp., sometimes written f.;
plural : formae speciales, ff. sp.) An intraspecific taxonomic
320
Francisella
Fort Bragg fever (pretibial fever) Human LEPTOSPIROSIS, caused
by Leptospira interrogans serotype autumnalis, which is characterized by a pretibial rash, malaise, coryza and fever; it occurs
in SE Asia, Japan, and the USA.
Fort Morgan virus See ALPHAVIRUS.
fortimicin An AMINOGLYCOSIDE ANTIBIOTIC which contains neither streptidine nor deoxystreptamine.
forward mutation A MUTATION which results in a mutant phenotype, i.e., a phenotype which differs from that of the WILD-TYPE
organism; a forward mutation typically involves the inactivation
of e.g. a structural gene. (cf. BACK MUTATION.)
forward primer In the context of a given gene whose nucleotides
are numbered: a primer whose sequence of nucleotides corresponds to a sequence within the gene which reads in a numerically ascending order in the 5 -to-3 direction; thus, a forward primer may have a sequence which corresponds to e.g.
nucleotides 10 25 (5 -to-3 ) of a given gene. The nucleotides
of a reverse primer read in a numerically descending order in
the 5 -to-3 direction e.g. nucleotides 350 335 in the other
strand.
fos See FBJ OSTEOSARCOMA VIRUS.
Foscarnet sodium See PHOSPHONOFORMIC ACID.
fosfomycin (phosphonomycin; cis-1,2-epoxypropyl-1-phosphonic
acid) A broad-spectrum ANTIBIOTIC (obtained from Streptomyces strains) which blocks PEPTIDOGLYCAN biosynthesis by
binding (irreversibly) and inhibiting phosphoenolpyruvate: UDPGlcNAc enolpyruvyl transferase thus preventing the synthesis
of N-acetylmuramic acid; other reactions involving PEP are
apparently not inhibited. Fosfomycin is taken up by the glycerolphosphate transport system in susceptible cells, and resistance to the drug develops readily by alteration or loss of this
transport system; plasmid-borne resistance involving intracellular modification of the drug also occurs [JGM (1985) 131
16491655].
Fosfonet sodium See PHOSPHONOACETIC ACID.
Foshay test A SKIN TEST in which the antigen is a suspension of
(or a protein extract from) killed cells of Francisella tularensis.
Foshays vaccine An anti-TULARAEMIA vaccine prepared from
killed cells of Francisella tularensis.
fossil microorganisms See e.g. COCCOLITH; CYANOBACTERIA;
DASYCLADALEAN ALGAE; FORAMINIFERIDA; GYROGONITES; RADIOLARIA; STROMATOLITES. (See also BIOSTRATIGRAPHY.) [Microfossils of the Proterozoic/Phanerozoic periods in China: Nature
(1985) 315 655658.]
foulbrood See AMERICAN FOULBROOD and EUROPEAN FOULBROOD.
Fourier transform See NUCLEAR MAGNETIC RESONANCE.
foveate Pitted with small holes or depressions.
foveolate Minutely pitted.
fowl adenovirus See AVIADENOVIRUS.
fowl cholera (avian pasteurellosis) A POULTRY DISEASE (affecting
e.g. chickens, turkeys, ducks, game birds) caused by Pasteurella
multocida. Symptoms of the acute form of the disease may
include anorexia, bloody diarrhoea, discharge from nostrils, eyes
and mouth, and haemorrhages of internal organs and mucous
membranes; death may occur within hours or days. In the chronic
form the disease mainly affects the respiratory system.
fowl paralysis Syn. MAREKS DISEASE.
fowl pest (1) Syn. FOWL PLAGUE. (2) Syn. NEWCASTLE DISEASE.
fowl plague A POULTRY DISEASE caused by strains of influenzavirus A. Symptoms resemble those of NEWCASTLE DISEASE;
mortality rates may be high. Wild birds may be an important
source of infection.
fowl pox A POULTRY DISEASE caused by an AVIPOXVIRUS. Infection
occurs via wounds (particularly in unfeathered regions such as
frange
in a cryoprotectant (e.g. 20% skim milk) to a cell density of
ca. 108 cells/ml. An aliquot of the suspension (ca. 0.1 ml) is
put into a sterile VIAL. (This account assumes the use of a vial
10 cm long, 6 mm internal diameter.) The COTTON WOOL plug
is replaced and pressed into the vial to a position ca. 23 cm
above the suspension. With precautions to avoid heating the
suspension, a region of the vial 23 cm from its open end is
heated and drawn out into a capillary neck. The suspension is
then frozen (see FREEZING) at 60 to 80 C, e.g. by placing
the closed end of the vial in a mixture of solid CO2 (dry ice)
and ethanol. The vial is transferred to a freeze-drying machine
(where the low temperature is maintained) and subjected to a
high vacuum for a period of 18 hours to several days, depending
on temperature. The vial is removed, fitted to a vacuum line,
and sealed by melting the capillary neck. Vials are best stored at
5 C or below. (For many species, viability is retained for 1030
years or longer.) When a culture is required, a vial is opened
and the contents reconstituted with broth or distilled water. A
sealed vial can be opened (preferably in a SAFETY CABINET) by
nicking the glass over the centre of the cotton wool plug and
momentarily applying a red-hot glass rod to the nick; the vial
(usually) cracks around its circumference, permitting the slow
ingress of air which is filtered through the cotton wool.
In the double-vial method, the material is freeze-dried in a vial
which is sealed only with a cotton wool plug; this vial is placed
in an outer vial, containing a desiccant, which is evacuated and
sealed by fusion of the glass.
freeze-etching A technique used for examining the topography
of surface(s) exposed by the fracture (cleavage) of e.g. a deepfrozen cell. The specimen is frozen rapidly (see FREEZING).
While at ca. 100 to 196 C (depending on apparatus), the
specimen is fractured: it may be split with a knife-blade in a
microtome-based apparatus, or, in one form of the snapped tube
apparatus, a capillary tube containing a homogenate is deepfrozen and snapped at a pre-scored position. During fracture,
part of the cleavage generally follows the boundaries of internal
structures (e.g. organelles), and membranes may be split to
expose their hydrophobic faces. Surfaces exposed by cleavage
are then etched by sublimation of volatiles (mainly water) from
the surfaces at a temperature of ca. 100 C under high vacuum;
organelles and non-volatiles are thus thrown into relief. A thin
replica of the etched surface is then prepared (see ELECTRON
MICROSCOPY (a)) and examined under the TEM. [Book ref. 4,
pp. 279341. For nomenclature of freeze-etched surfaces see
Science (1975) 190 5456. For potential artefacts see JUR
(1983) 82 123133.]
freeze-fracturing The process of FREEZE-ETCHING omitting the
etching step.
freeze pressing The operation of a HUGHES PRESS.
freeze-sectioning (cryosectioning) The preparation of sections,
for MICROSCOPY or ELECTRON MICROSCOPY, by cutting a FROZENHYDRATED SPECIMEN with a cryotome (a modified MICROTOME
which maintains the specimen in a frozen state).
freeze-substitution A procedure for preparing a specimen e.g.
for X-RAY SPECTROCHEMICAL ANALYSIS. Essentially, the specimen
is rapidly frozen and then immersed for e.g. 14 days in anhydrous
ethanol or acetone at e.g. 70 C; during this time the ice is
gradually replaced by ethanol or acetone. This method helps
to maintain the positions of e.g. water-soluble ions within the
specimen thus facilitating subsequent determination of the in
vivo locations of these ions.
freezing Sub-zero ( C) freezing is used for the preservation
(cryopreservation) of certain microorganisms, foods etc, and
Friend virus
e.g. in
FREEZE-DRYING
and
FREEZE-ETCHING
CRYOFIXATION).
Frings Acetator
fruit spoilage See e.g. CANNING; GREY MOULD; PECTIC ENZYMES;
PICKLING; SOFT ROT (2).
fruiting body (fructification; fruit body; sporocarp) Any specialized structure (plectenchymatous in fungi) which bears or contains sexually- or asexually-derived spores. Examples include
e.g. APOTHECIUM, PYCNIDIUM, pycnium and the resting structures
of the MYXOBACTERALES. Some fruiting bodies (e.g. those formed
by species of Heterobasidion and Poria) are perennial.
frustule See DIATOMS.
fruticose Shrub-like. Of a LICHEN: having a thallus which is
thread-like (terete) or strap-like (more or less flattened) and
either erect and shrubby or pendulous; the thallus may be
attached to the substratum by a holdfast or may be unattached.
The mechanical strength of the thallus may derive from a dense
axial strand (in USNEA) or from the cortex; thalli of the latter
type may or may not be hollow. (cf. CRUSTOSE; FOLIOSE.)
FTA-ABS test (fluorescent treponemal antibody-absorption test)
A TREPONEMAL TEST used in the diagnosis of SYPHILIS. Initially,
the patients serum is absorbed with an extract of Reiter treponemes to remove non-specific anti-treponemal antibodies, and
the absorbed serum is applied to a slide on which there is a film
of killed, fixed cells of Treponema pallidum; the slide is then
briefly incubated to allow any specific antibodies in the serum
to combine with the surface antigens of T. pallidum. The slide
is rinsed free of serum and briefly re-incubated with fluorescent
conjugate (anti-human globulin conjugated with a fluorescent
dye); uncombined conjugate is rinsed off and the slide is examined by fluorescence MICROSCOPY. Antibodies which combine
with T. pallidum combine also with the conjugate their presence being indicated by fluorescent treponemes.
FTO agar A selective medium used for the culture of Micrococcus spp. It consists of trypticasesoy agar containing 0.1%
yeast extract, 0.5% Tween 80, and small amounts of furoxone
and Oil Red O. [Preparation and use: Book ref. 46, p. 1542.]
ftsA gene (Caulobacter) See CAULOBACTER.
FtsH An ATP- and zinc-dependent protease within the cytoplasmic membrane of Escherichia coli and many other bacteria; it
is encoded by gene ftsH (also called hflB and tolZ ). In E. coli,
FtsH is involved e.g. in the degradation of certain membrane and
regulatory proteins (including the HEAT-SHOCK PROTEIN s32 ), and
it may also act as a chaperone. [FtsH (review): FEMS Reviews
(1999) 23 111.]
ftsI gene See PENICILLIN-BINDING PROTEINS.
ftsQ gene (Caulobacter) See CAULOBACTER.
FtsY protein See PROTEIN SECRETION (type II systems).
ftsZ gene See SOS SYSTEM.
FtsZ protein See CELL CYCLE (b) and SOS SYSTEM.
5-FU 5-Fluorouracil (see e.g. PHENOTYPIC SUPPRESSION).
fuberidazole (2-(2 -furyl)-benzimidazole) An agricultural antifungal agent (see BENZIMIDAZOLES); it is particularly useful as
a seed treatment for the control of Fusarium infections (e.g.
F. nivale in cereals).
Fucales See FUCUS and PHAEOPHYTA.
fucan A polymer of FUCOSE. (See also FUCOIDIN.)
fuchsin (fuchsine) Basic fuchsin is a red-purple DYE consisting
mainly of pararosanilin and rosanilin (see TRIPHENYLMETHANE
DYES). (See also CARBOLFUCHSIN and BRUCELLA.) Acid fuchsin,
derived from basic fuchsin by sulphonation, is used e.g. in
ANDRADES INDICATOR.
fucidin See FUSIDIC ACID.
fucoidin (fucoidan; fucan) A group of complex, branched, sulphated heteropolysaccharides present in phaeophycean algae;
fucoidins contain fucose (usually sulphated), xylose, glucuronic
fungi
under aerobic conditions and repressed under anaerobic conditions. Fumarate reductase is bound to the cytoplasmic face of the
cytoplasmic membrane [JGM (1984) 130 28512855]; fumarate
respiration thus requires a fumarate transport system. Fumarate
reductase in E. coli consists of an FAD-containing protein subunit (frdA gene product), an ironsulphur protein subunit (frdB
gene product), and two small, hydrophobic anchor proteins
(frdC and frdD gene products) which anchor the enzyme in
the membrane; these four cistrons occur in an operon with a
promoteroperator region and a transcriptional terminator. The
energy yield of fumarate respiration in E. coli is uncertain, but
has been calculated to be ca. 0.66 ATP/fumarate [MR (1984) 48
222271].
In Wolinella succinogenes, fumarate is used as an electron acceptor for the oxidation of formate (HCOO + H+ +
fumarate succinate + CO2 ) or H2 , yielding, by oxidative
phosphorylation, 12 ATP per fumarate reduced.
fumigant See FUMIGATION.
fumigation The exposure of an enclosed space (e.g. a horticultural glasshouse, a hospital room) to a gaseous or vapour-phase
DISINFECTANT or STERILANT. Control of humidity is commonly
important for effective fumigation. Agents used for fumigation
(fumigants) include e.g. DAZOMET, ETHYLENE OXIDE, FORMALDEHYDE, SULPHUR DIOXIDE.
fumitremorgin A tremorgenic MYCOTOXIN produced e.g. by
Aspergillus fumigatus and Penicillium piscarium.
functional immunity Syn. IMMUNITY (3).
fungaemia (fungemia) The presence of fungi in the bloodstream.
fungemia See FUNGAEMIA.
fungi (sing. fungus) Unicellular, multicellular or coenocytic, heterotrophic, eukaryotic MICROORGANISMS which do not contain
chlorophyll (cf. ALGAE) and which characteristically form a rigid
CELL WALL containing CHITIN and/or CELLULOSE (cf. PROTOZOA).
In some taxonomic schemes [see e.g. Book ref. 64] the fungi are
divided into two divisions: EUMYCOTA (true fungi) and MYXOMYCOTA; since members of the Myxomycota are commonly
regarded as protozoa, the following account refers specifically
to the true fungi.
In most fungi the vegetative form (thallus) consists of
hyphae (see HYPHA), while in e.g. many YEASTS the thallus is
predominantly or exclusively unicellular (cf. DIMORPHIC FUNGI).
(See also GROWTH (fungal).) The majority of fungi are nonmotile; however, flagellated reproductive/disseminative forms
are produced by many of the LOWER FUNGI. (Phylogenetically,
motility is regarded as a primitive feature among the fungi.)
Most fungi can reproduce asexually often by the formation
of conidia (see CONIDIUM). In sexual reproduction, interaction
between individuals may involve e.g. anisogamy, GAMETANGIAL CONTACT, isogamy, oogamy (see MONOBLEPHARIDALES), or
SOMATOGAMY. (See also PARASEXUAL PROCESSES.) Specialized
asexual and/or sexual SPORE-bearing structures (see e.g. FRUITING BODY) are formed by most fungi; many are macroscopic,
and some (e.g. the mushrooms and puffballs) may be several
centimetres or more in size.
Fungi are osmotrophic chemoheterotrophs which, collectively,
utilize substrates ranging from simple sugars to e.g. cellulose (see CELLULASES), HYDROCARBONS, LIGNIN, pectins (see
PECTIC ENZYMES) and xylans (see XYLANASES). Energy-yielding
metabolism may involve RESPIRATION and/or FERMENTATION.
Although fungi are typically aerobic organisms, some are facultative or obligate anaerobes (see e.g. RUMEN).
The fungi are widespread in nature; most species are terrestrial, but some (see e.g. NIA, OOMYCETES, SPATHULOSPORALES) are
Fungi Imperfecti
funicular cord See CYATHUS.
funiculus See CYATHUS.
funoran A mucilaginous sulphated galactan produced by
Gloiopeltis furcata; it consists mainly of D-galactose and 3,6anhydro-L-galactose residues, with some L-galactose residues.
In Japan, funoran is used as an adhesive and sizing agent.
Fur protein A multifunctional regulatory protein encoded by
the fur gene. In many bacteria, Fur is involved e.g. in the
control of ferric iron uptake (hence ferric uptake regulator); for
example, after uptake of adequate ferric iron in Escherichia coli,
accumulated intracellular ferrous ions cause the Fur protein to
repress transcription from various genes (e.g. fep genes) which
encode cell envelope proteins involved in ferric iron uptake.
Repression involves the binding of Fe2+ Fur to an operator
sequence (the iron box) upstream of the coding region in the
affected genes. (See also OPERATOR.) Fur has many functions
other than iron regulation e.g. in Salmonella typhimurium
it is involved in the acid tolerance response [JB (1996) 178
56835691].
furacin Nitrofurazone: see NITROFURANS.
furadantin Nitrofurantoin: see NITROFURANS.
furalaxyl See PHENYLAMIDE ANTIFUNGAL AGENTS.
furaltadone See NITROFURANS.
furamide See DILOXANIDE.
furazlocillin A b-LACTAM ANTIBIOTIC which binds exclusively to
PBP-3 (see PENICILLIN-BINDING PROTEINS).
furazolidone See NITROFURANS.
furcellaran (Danish agar) A sulphated galactan, similar to kCARRAGEENAN, isolated from Furcellaria fastigiata; it has been
used as a gelling agent in the food industry.
Furcellaria See RHODOPHYTA.
furfuraceous Scurfy; covered with small scales.
furocoumarin Syn. PSORALEN.
furoviruses See SOIL-BORNE WHEAT MOSAIC VIRUS.
furoxone Furazolidone: see NITROFURANS.
furuncle Syn. BOIL.
furunculosis (1) A FISH DISEASE affecting mainly freshwater fish,
particularly salmonids. Pathogen: Aeromonas salmonicida. The
typical disease occurs in two forms. In the acute form external
symptoms are usually absent; internal organs become inflamed
and haemorrhagic, and death is usually rapid. In the subacute
form furuncle-like swellings (containing necrotic tissue, blood
and bacteria) appear on the body. A chronic, subclinical carrier
state is also known. Infection may occur via gills or wounds;
high temperature (1219 C) is a predisposing factor. Atypical
forms of the disease (ulcerative furunculosis), caused by
atypical strains of A. salmonicida, occur in salmonids and nonsalmonids (e.g. goldfish) and involve progressive ulceration of
skin and underlying muscle. (cf. ULCER DISEASE.)
A. salmonicida produces several extracellular toxins, including a leucocytolytic factor, proteases (caseinase and gelatinase), and two haemolysins: H-lysin and T-lysin; H-lysin is a
broad-spectrum haemolysin [purification and properties: JGM
(1985) 131 16031609], while T-lysin appears to be active
specifically against trout RBCs. These products may, together,
play a role in the pathogenicity of A. salmonicida.
(2) (med.) The (simultaneous or sequential) formation of a
number of BOILS.
furylfuramide (AF-2) See NITROFURANS.
fusarenon-X See TRICHOTHECENES.
fusaric acid (2-carboxyl-5-n-butylpyridine) A TOXIN produced
sometimes together with dehydrofusaric acid and 10-hydroxyfusaric acid by several species of Fusarium. It apparently
fusion protein
eye infections and skin lesions in man and animals; such infections are usually or always secondary to trauma or debilitation
in the host.
In immunocompromised patients, invasive infection by Fusarium may mimic aspergillosis; a PCR-based examination may be
useful for detecting this organism in clinical specimens [JCM
(1999) 37 24342438].
Fusarium spp have been used commercially as sources of
ENNIATINS, GIBBERELLINS for horticultural use, ZEARALENONE
derivatives for medical and veterinary use, and in the production
of single-cell protein. (See also PAPER SPOILAGE and TIMBER
STAINING.)
[Applied aspects: Book ref. 131.]
fusarium wilt A VASCULAR WILT caused by a Fusarium sp
usually F. oxysporum (oxysporum wilt). Strains of F. oxysporum may have a narrow, intermediate or wide host range:
e.g. F. oxysporum f. sp. cubense infects banana plants (Panama
disease); f. sp. lini infects flax; f. sp. lycopersici infects
tomatoes (cf. LYCOMARASMIN); f. sp. conglutinans infects
cruciferous plants; f. sp. vasinfectum infects e.g. coffee, cotton,
cowpea, rubber (Hevea), soybean, and many other plants.
Typical symptoms of fusarium wilts include brown or black
vascular discoloration and wilting, sometimes preceded by
e.g. epinasty, vein-clearing and leaf chlorosis; affected plants
generally die.
fusarubin See NAPHTHAZARINS.
Fuscidea See LECIDEA.
fusel oil A mixture of higher alcohols (mainly amyl, isoamyl,
isobutyl, and propyl alcohols) formed in small quantities as byproducts of ALCOHOLIC FERMENTATION; the alcohols are formed
by deamination, decarboxylation and reduction of amino acids,
and from keto acid precursors of amino acids.
fusicoccin A toxin, produced by Fusicoccum amygdali, which
can affect a range of plants. Fusicoccin can increase the rate
at which a plant loses water, e.g. by promoting the opening of
stomata. It can also stimulate H+ efflux across the plasmalemma,
thus facilitating uptake of e.g. K+ and certain energy-yielding
substrates; this may at least partly account for the observed
growth-promoting activity of fusicoccin.
Fusicoccum A genus of fungi of the COELOMYCETES.
fusidic acid An ANTIBIOTIC synthesized e.g. by Cylindrocarpon
spp (= Fusidium coccineum) and Acremonium (Cephalosporium) spp; it is a steroid structurally related to cephalosporin
P1 with which it exhibits cross-resistance. Sodium fusidate
(fucidin) is active (bacteriostatic) against Gram-positive bacteria,
particularly staphylococci; it inhibits PROTEIN SYNTHESIS by binding to EF-G, preventing the dissociation of EF-G and GDP from
the ribosome following translocation. The EF-Gs (= EF-2s) of
certain archaeans (e.g. methanogens, halobacteria) are sensitive
to fusidic acid, whereas those from e.g. Desulfurococcus mobilis,
Sulfolobus solfataricus, Thermococcus celer and Thermoplasma
acidophilum are insensitive [JB (1986) 167 265271].
Fusidium See CYLINDROCARPON.
fusiform Spindle-shaped: tapered at both ends.
Fusiformis An obsolete bacteria genus. (See BACTEROIDES and
FUSOBACTERIUM.)
fusigen A SIDEROPHORE produced by e.g. Aspergillus spp.
fusion protein (1) In e.g. viruses of the genus PARAMYXOVIRUS
(e.g. Sendai virus): a protein which promotes fusion between
host cells, as well as between virus envelope and cell membrane.
(2) (biotechnol.) A protein containing amino acid sequences
from each of two distinct proteins; it is formed by the expression
of a recombinant genetic construct prepared by joining together
Fusobacterium
useful experimental approach, certain reporter genes have been
found to influence the activity of some promoters [JB (1994)
176 21282132].
(Fusion protein is also used to refer to the products of certain
viral ONCOGENES e.g. MYC.)
Fusobacterium
A genus of Gram-negative bacteria (family
BACTEROIDACEAE) which occur e.g. in the human mouth and
intestine, and in the RUMEN, and which include human and animal
pathogens (see NECROBACILLOSIS and FOOT-ROT; see also SWINE
DYSENTERY). Cells: typically fusiform or non-fusiform rods or
filaments; all species are non-motile. Fermentation of peptone or
carbohydrates yields butyric acid as a major product; isobutyric
and isovaleric acids are not formed, but small amounts of acetic,
formic, lactic or propionic acids may be formed. Optimum
growth temperature: ca. 37 C. GC%: ca. 2634. Type species:
F. nucleatum.
F. necrophorum (formerly Fusiformis necrophorus, Sphaerophorus necrophorus). Fusiform or round-ended cells. Propionate
is formed from both threonine and lactate; aesculin is not
hydrolysed; indole +ve; copious gas is usually formed from
glucose.
F. nucleatum (formerly Fusiformis fusiformis, Fusobacterium
polymorphum, Sphaerophorus fusiformis). Cells: typically
fusiform rods or filaments. Propionate is formed from threonine
but not from lactate; aesculin is not hydrolysed; indole +ve;
typically, little gas is formed from glucose.
Other species: F. gonidiaformans, F. mortiferum, F. naviforme, F. necrogenes, F. perfoetens, F. prausnitzii, F. russii and
F. varium.
Fusulina See FORAMINIFERIDA.
fusulinids See FORAMINIFERIDA.
Fusulinina See FORAMINIFERIDA.
futile cycle The cyclic interconversion of two compounds by
irreversible reactions catalysed by two or more enzymes
which are active at the same time within a given cell, the
result being an apparently useless dissipation of energy. For
example, in e.g. Escherichia coli phosphofructokinase catalyses ATP-dependent phosphorylation of fructose 6-phosphate to
fructose 1,6-bisphosphate [see Appendix I(a)], and fructose bisphosphatase hydrolyses fructose 1,6-bisphosphate to fructose 6phosphate and inorganic phosphate (Pi) (see GLUCONEOGENESIS);
if both enzymes were to be active simultaneously, the net result
would be the hydrolysis of ATP to ADP + Pi. Presumably, futile
cycles are normally prevented by control of the presence/activity
of enzymes with opposing functions; however, they may have a
role under certain conditions: e.g., it has been suggested that a
futile cycle that results in ATP hydrolysis could provide Pi from
endogenous ATP when the exogenous supply of Pi is interrupted
[ARM (1984) 38 459486 (471473)].
FV3 FROG VIRUS 3.
328
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
G
G (1) Guanine (or the corresponding nucleoside or nucleotide)
in a nucleic acid. (2) Glycine (see AMINO ACIDS).
G-actin See ACTIN.
(G + C)% value See GC%.
G loop If the DNA of BACTERIOPHAGE MU is extracted from
virions obtained by induction of a lysogenic population of
bacteria and is then denatured and re-annealed, a proportion
of the resulting dsDNA molecules show a bubble or loop of
unpaired strands in the G region of the DNA; this loop the G
loop reflects localized non-homology generated by inversion
of the G segment during lysogeny. (G loops are rarely observed
in phage DNA derived from lytic infections.)
G phases (of cell cycle) See CELL CYCLE.
G proteins (GTP-binding proteins) In eukaryotic cells: GTPbinding proteins involved mainly in intracellular signalling.
There are two main types of G protein: (i) the heterotrimeric
type (each G protein consisting of a, b and g subunits), and (ii)
the (smaller) proteins of the Ras superfamily (= p21 family).
Heterotrimeric G proteins are characteristically associated
with the cytoplasmic domain of certain transmembrane receptors
(e.g. the receptors for CHEMOKINES). (See also ADENYLATE
CYCLASE.) In the inactive state, a GDP residue binds to the
a subunit of the protein. During activation of the G protein
(through receptorligand binding), the a subunit separates from
the other two subunits (which stay together), and GDP on the a
subunit is exchanged for GTP; when activated in this way (i.e.
when binding GTP), the a subunit can behave as an effector
molecule in the signalling pathway as can the b + g entity.
During de-activation of the G protein, GTPase activity (inherent
in the a subunit) cleaves the terminal phosphate from GTP so
that the a subunit is then bound to GDP; the a subunit (with
bound GDP) then re-associates with b + g to form the inactive
G protein.
G proteins of the Ras superfamily interact with several
factors during their cycle of activation and de-activation. During
activation, a guanosine nucleotide exchange factor promotes the
exchange of (bound) GDP for GTP; the activated G protein (i.e.
with bound GTP) can then act as an effector molecule in the
signalling pathway. During de-activation, a GTPase-activating
factor stimulates the latent GTPase activity of the G protein,
thus giving rise to the inactive (GDP-bound) state. Another
factor guanosine nucleotide dissociation inhibitor inhibits
the exchange of GDP for GTP.
G1 -event model See CELL CYCLE.
Gaeumannomyces A genus of fungi of the order DIAPORTHALES.
G. graminis (formerly Ophiobolus graminis), the causal agent
of TAKE-ALL, forms dark, thick-walled perithecia which occur
immersed in leaf sheaths and stem bases with their beaks
(i.e., necks) protruding; the ascospores are septate, filiform or
fusiform. (See also MYCOVIRUS.)
Gaeumannomyces graminis virus See MYCOVIRUS.
gaffkaemia (gaffkemia) A fatal septicaemic disease of lobsters (Homarus spp) caused by Aerococcus viridans (formerly
Gaffkya homari ); infection occurs via breaks in the integument.
Gaffkya An obsolete bacterial genus [nom. rejic. IJSB (1971) 21
104105]. (See also AEROCOCCUS and PEPTOSTREPTOCOCCUS.)
gag gene See RETROVIRIDAE.
gal operon See OPERON and OPERATOR.
galactan
A polymer of
GALACTOSE:
see e.g.
AGAR; AMYLOVORIN;
329
galvanotaxis
Bacterium-induced galls include e.g. CROWN GALL, FASCIATION
(some instances), HAIRY ROOT, and OLIVE KNOT; galls can also be
induced by Erwinia herbicola. (See also ROOT NODULES.)
Fungus-induced galls (mycocecidia) include e.g. CLUBROOT,
WART DISEASE and WITCHES BROOM; galls are also induced by
e.g. Albugo candida on certain crucifers, by some smut fungi
(see SMUTS sense 2), and by members of the EXOBASIDIALES.
(See also cedar apples under GYMNOSPORANGIUM.)
Virus-induced galls include those caused by the RICE GALL
DWARF VIRUS and the WOUND TUMOUR VIRUS. (See also ENATIONS
and FIJI DISEASE.)
galvanotaxis A TAXIS in which the stimulus is an electrical potential gradient. An organism may move (with its anterior end
pointing in the direction of motion as in normal motility) towards
the cathode (negative galvanotaxis) or anode (positive galvanotaxis). Paramecium is said to be negatively galvanotactic, but
with a higher potential difference it may move towards the anode
with its (normally) posterior end leading. Some protozoa are
positively galvanotactic.
Gambierdiscus See CIGUATERA.
gametangial contact (gametangy) A process in which one or
more male nuclei pass from a male gametangium to a female
gametangium either (according to species) via a pore which
develops at the point of contact of the two gametangia, or via a
TRICHOGYNE which grows between the gametangia.
gametangial copulation The occurrence of plasmogamy and
karyogamy in a process which may involve either the complete
fusion of two gametangia (gametangial fusion) or the transfer
of the contents of one gametangium into the other.
gametangial fusion See GAMETANGIAL COPULATION.
gametangium A structure which gives rise to gametes or which,
in its entirety, functions as a gamete.
gametangy Syn. GAMETANGIAL CONTACT.
gamete A haploid cell or nucleus involved in sexual reproduction during which two gametes fuse to form a zygote. (See
also ANISOGAMY; ISOGAMY; OOGAMY.)
gametic meiosis MEIOSIS, in a meiocyte other than a zygote,
preceding gamete formation in a life cycle in which DIPLOPHASE
predominates. (cf. ZYGOTIC MEIOSIS.)
gametocytaemia The presence in the bloodstream of gametocyte
stages of a parasite.
gametocyte Any cell which gives rise to gamete(s); a gametocyte
may be haploid (see ALTERNATION OF GENERATIONS) or diploid
(see GAMETIC MEIOSIS).
gametogony (gamogony) (1) The formation of gametocytes and
gametes. (2) The formation of gametes from gametocytes.
gametophyte See ALTERNATION OF GENERATIONS.
gametothallus See ALTERNATION OF GENERATIONS.
gamma chain (immunol.) See HEAVY CHAIN.
gamma-delta (gd) See entry Tn3.
gamma globulins A subclass of serum globulins (which includes
the IMMUNOGLOBULINS) characterized by low electrophoretic
mobility towards the anode or, under certain conditions, movement towards the cathode (see ELECTROENDOSMOSIS).
gamma interferon See INTERFERONS.
gamma particle (1) See PSEUDOCAEDIBACTER. (2) (mycol.) In the
zoospores of some members of the Chytridiomycetes (e.g.
Blastocladiella emersonii ): an ovoid particle, one or more
of which appear to play a role in cyst wall formation; in
B. emersonii the gamma particles (each ca. 500 nm diam.)
exhibit chitin synthase activity. [Book ref. 175, pp. 544545.]
gamma-rays (g-rays) See IONIZING RADIATION.
Gammacell A laboratory apparatus used as a source of gammaradiation. (See also IONIZING RADIATION.)
gasteroid
gangrene results from a gradual reduction in local blood supply,
with darkening, drying and shrivelling of the tissues. Moist
gangrene is sudden in onset, resulting e.g. from injury followed
by bacterial infection and putrefaction; it may spread very
rapidly. (cf. GAS GANGRENE; see also e.g. ERGOTISM.)
(2) (plant pathol.) A disease of stored potato tubers, caused
by Phoma exigua (e.g. var. foveata in the UK), in which the
tubers become decayed and hollow. Surface contamination of
the tubers occurs during harvesting, an important source of the
pathogen being pycnidia from senescent potato stems; infection
occurs via wounds made during or after harvesting. The disease
may be controlled with e.g. benomyl or thiabendazole. (See also
POTATO DISEASES.)
gangrenous coryza Syn. MALIGNANT CATARRHAL FEVER.
Ganoderma See APHYLLOPHORALES (Ganodermataceae).
Ganodermataceae See APHYLLOPHORALES.
gap (in dsDNA) See NICK.
GAR-936 See TETRACYCLINES.
GardnerArnstein feline sarcoma virus See FES.
Gardnerella
A genus (incertae sedis) of catalase-negative,
oxidase-negative, chemoorganotrophic, apparently Gram typenegative bacteria which occur in the human genital and urinary
tracts and which are commonly associated with BACTERIAL
VAGINOSIS. Cells: pleomorphic rods, ca. 0.5 1.52.5 m. The
genus includes both obligately anaerobic and facultatively
anaerobic strains. The organisms are nutritionally fastidious:
little or no growth occurs on nutrient agar. Neither X FACTOR
nor V FACTOR is required. Growth occurs e.g. on certain bloodcontaining media and on peptonestarch D-glucose medium;
most strains can grow aerobically on blood agar at 35 C.
Clear (b) haemolysis occurs on human (but not sheep) blood
plates. Most strains ferment maltose (and some ferment lactose)
forming acid but not gas. Nitrate is not reduced. Optimum
growth temperature: 3537 C. GC%: ca. 4244. Type species:
G. vaginalis (formerly Haemophilus vaginalis). [Book ref. 22,
pp. 587591.]
Gardneriella See RHODOPHYTA.
gari A West African food made by the fermentation of cassava
pulp. The essential organisms appear to be Leuconostoc and
Candida spp.
gas bladder (algol.) Syn. PNEUMATOCYST.
gas gangrene A type of acute, rapidly spreading GANGRENE
(sense 1) which typically results from the infection of a wound
with certain anaerobic bacteria, particularly Clostridium spp
(e.g. C. perfringens type A, C. septicum, C. novyi ); these organisms produce a variety of extracellular enzymes (see CLOSTRIDIUM) which promote tissue destruction. The a-toxin of Clostridium perfringens (which hydrolyses lecithin and also has sphingomyelinase activity) appears to be the major lethal toxin
[Mol. Microbiol (1995) 15 191202]. Gas gangrene may occur
in e.g. subcutaneous tissues (clostridial CELLULITIS), muscle
(clostridial myonecrosis), or internal organs. Infected tissues
become necrotic, discoloured, and swollen with serosanguinous
fluid and pockets of gas (hydrogen, carbon dioxide) produced
by the clostridia; the gas exerts pressure on adjacent tissues,
further disrupting the blood supply to these tissues and promoting spread of the gangrene. Treatment: e.g. surgery; antibiotic
therapy; treatment with hyperbaric oxygen. (Other organisms
occasionally implicated in gas gangrene include anaerobic streptococci and Escherichia coli ; mixed infections also occur.)
gasliquid chromatography See CHROMATOGRAPHY.
gas vacuole A subcellular organelle, found only in prokaryotes,
which consists of clusters of hollow, cylindrical, gas-filled vesicles (gas vesicles). Gas vacuoles appear bright and refractile
under the light microscope. They occur in planktonic cyanobacteria, particularly bloom-forming species (e.g. Anabaena flosaquae, Trichodesmium), and in certain archaeans and bacteria
(e.g. strains of Halobacterium, Methanosarcina, Pelodictyon and
Rhodopseudomonas).
In cyanobacteria, gas vacuole formation is usually constitutive, but it may be inducible in hormogonia (see HORMOGONIUM).
The gas vesicles of cyanobacteria are hollow cylinders with
conical ends; they are ca. 60250 nm in diameter and of
variable length (e.g. 300 nm); they have a ribbed construction.
Vesicles from other prokaryotes (including Methanosarcina) are
generally similar in both morphology and construction (although
they may differ in size), but those of Halobacterium are usually
spindle-shaped.
Vesicles are composed of a rigid monolayer of a single type of
protein (gas vesicle protein GVP); they are permeable to gases
but not to water. GVPs from e.g. cyanobacteria and halobacteria
show some homology [JGM (1984) 130 27092715].
The primary function of a gas vacuole is to give buoyancy
to the (free-floating) organism. Gas vesicles collapse when
subjected to pressure (ca. 5 atmospheres for many freshwater
cyanobacteria, ca. 50 atmospheres for Trichodesmium). The
vesicles in some freshwater species can be collapsed by high
turgor pressures within the cells, thus providing a mechanism
whereby these cells can regulate their buoyancy and, hence,
their position in the water: an increase in light intensity
causes an increase in turgor pressure in the cell (due to lightstimulated accumulation of potassium ions and the accumulation
of photosynthate), resulting in the collapse of part of the gas
vacuole and hence loss of buoyancy. New gas vesicles form
when the light intensity is low, thus increasing buoyancy.
(There is some evidence that the GVP of collapsed vesicles
disaggregates and may be re-used in the assembly of new
vesicles [JGM (1984) 130 15911596].)
Another mechanism for the regulation of buoyancy occurs e.g.
in Oscillatoria agardhii and in a strain of Microcystis [JGM
(1985) 131 799809]: when the intensity of light is high, gas
vesicles do not collapse but existing vesicles are diluted out
by cell growth and division.
gas vesicle (1) See GAS VACUOLE. (2) Syn. PNEUMATOCYST.
gasohol A mixture of gasoline and (up to ca 20% v/v) ethanol
which is used as a fuel. (See also INDUSTRIAL ALCOHOL.)
GasPak An ANAEROBIC JAR which consists of a strong, cylindrical, transparent plastic (polycarbonate) chamber with a flat,
gas-tight lid which is secured by means of a screw clamp. The
jar is loaded (with e.g. plates), and an indicator of anaerobiosis
(e.g. a pad soaked with a METHYLENE BLUE solution) is placed
inside the jar. Water is then added to a small foil sachet containing (i) sodium borohydride and (ii) a mixture of powdered
sodium bicarbonate and citric acid which (with water) yield
H2 and CO2 , respectively; the sachet is quickly placed in the jar
in an upright position and the lid is clamped in place. Attached
to the inside of the lid is a cold catalyst (see MCINTOSH AND
FILDES ANAEROBIC JAR) which promotes the elimination of O2 .
Anaerobiosis within the jar develops within a few hours. Since
this type of jar does not require evacuation, plates can be incubated upside down (i.e. lid-side down); this avoids the problem
(which can arise with the McIntosh and Fildes jar) in which
water of condensation drops from the inside of the Petri dish lid
onto the agar surface.
gasteroid Refers to the type of fruiting body which is characteristic of fungi of the GASTEROMYCETES: angiocarpic, forming
STATISMOSPORES. (cf. AGARICOID.)
331
gasteroid basidiospore
gasteroid basidiospore A term proposed for a BASIDIOSPORE
which is not forcibly discharged from the basidium [BBMS
(1983) 17 8294 (86)]. (cf. STATISMOSPORE.)
Gasteromycetes A class of fungi (subdivision BASIDIOMYCOTINA)
characterized by the formation of epigean or hypogean, sessile or
stipitate basidiocarps which undergo ANGIOCARPIC DEVELOPMENT
and give rise to STATISMOSPORES. The typical basidiocarp consists
of e.g. fleshy or cartilaginous fertile tissue (the GLEBA) enclosed
by a limiting wall (PERIDIUM); in some species the basidiocarp
contains a definite hymenium, while in others the fertile cells
are scattered, singly or in groups, throughout the spore-bearing
tissue. (See also CAPILLITIUM.) The dispersal of mature basidiospores depends e.g. on the disintegration or perforation of the
peridium. Gasteromycetes occur typically as saprotrophs on soil,
dead wood and dung; some species form mycorrhizal associations.
The orders [Book ref. 64, p. 160] are:
Gautieriales. Hymenium-forming, hypogean saprotrophs or
mycorrhizal fungi.
Hymenogastrales. Hymenium-forming, typically hypogean
saprotrophs, mycorrhizal fungi and parasites. Some authors
include gasteroid members of the Russulales in this order. Genera include e.g. Hymenogaster and Rhizopogon (which forms
mycorrhizal associations with conifers).
LYCOPERDALES (q.v.).
Melanogastrales. Hypogean or marine; mature gleba mucilaginous, lacking a true hymenium. Genera include Melanogaster
and NIA.
NIDULARIALES (q.v.).
PHALLALES (q.v.).
Podaxales. An order which includes some of the SECOTIOID
FUNGI.
SCLERODERMATALES (q.v.).
Tulostomatales. An order which includes the stipitate puffballs
(e.g. Battarrea, Calostoma).
gastric flu A term sometimes used to refer to the syndrome
caused by infection with Influenzavirus type B in which some
studies have recorded involvement of the gastrointestinal tract.
gastriole Syn. FOOD VACUOLE.
gastroenteritis Inflammation of the lining of the stomach and
intestine (usually the small intestine), usually resulting in DIARRHOEA and vomiting. (cf. ENTERITIS.) It may be due e.g. to allergic
reactions, chemical poisoning (e.g. by excessive alcohol consumption), or to microbial infection or toxins (see e.g. FOOD
POISONING).
gastrointestinal tract flora The mammalian gastrointestinal tract
is normally sterile at birth, but thereafter becomes rapidly
colonized by a range of bacteria. The gut flora of the human
infant initially includes Lactobacillus and Bifidobacterium spp,
coliforms and clostridia, but the flora depends to some extent on
diet: the gut of breast-fed infants contains a higher proportion
of bifidobacteria and lactobacilli and fewer coliforms than
that of infants bottle-fed on cows milk [Book ref. 107,
pp 126]. Acid production by the lactic acid bacteria is believed
to discourage the growth of enterobacteria, including enteric
pathogens. On weaning, the gut flora becomes more complex
and soon resembles that of the adult.
In adult humans, many of the bacteria ingested with food (and
oral bacteria swallowed with saliva) are killed by the acidity in
the stomach. However, despite the normal acidity of the stomach,
it appears that this region of the gut is colonized by Helicobacter
pylori (see HELICOBACTER) in a high proportion of the human
population. (A greater number and variety of organisms may be
present in the stomach in cases of achlorhydria.)
geminiviruses
and provide a useful criterion in microbial TAXONOMY; however,
a similarity in GC% values, by itself, does not necessarily
indicate a close taxonomic relationship. The possession of
a PLASMID (particularly one with a high copy number) may
affect the observed GC% value of a cell unless the method
used for extracting chromosomal DNA discriminates against
extrachromosomal nucleic acids.
The GC% of a DNA sample may be obtained, indirectly,
by determining its melting point (Tm : see THERMAL MELTING
PROFILE), since Tm is linearly related to GC% (i.e., a high Tm
correlates with a high GC%). Alternatively, an indirect determination of GC% may be achieved by buoyant density (Bd)
measurement (e.g. in a CsCl density gradient see CENTRIFUGATION) since Bd is also linearly related to GC%.
GC% values in bacteria fall within the approximate range
2575; as a guideline, intra-species variation should be not more
than 45% and intra-genus variation not more than 10% [Book
ref. 59, p. 14].
[Methods for determining DNA base composition: Book
ref. 138, pp. 131.]
GC type See BASE RATIO.
GDP Guanosine 5 -diphosphate.
Geastrum See LYCOPERDALES.
gel diffusion In serology: gel diffusion (= immunodiffusion)
refers to any procedure in which antibodies (usually in an
antiserum) and/or antigens diffuse through a gel medium (e.g.
AGAR or agarose) forming a precipitate in the gel where
homologous (or cross-reacting) antigens and antibodies meet
in OPTIMAL PROPORTIONS. (Agar/agarose at concentrations of ca.
0.5% to 1.5% allows the diffusion of antibody-sized molecules
but hinders random mechanical and thermal movements in the
medium.) Lines, bands or haloes of whitish precipitate are
obtained (within hours or a day or two) in number(s) and
position(s) which depend on the number and nature of the
homologous (or cross-reacting) pairs of antigens and antibodies
within the diffusing system. The precipitate may or may not be
visible to the naked eye; visibility may be enhanced by washing
the gel free of uncombined antigen and antibody, and staining the
precipitate in situ with a protein stain (e.g. COOMASSIE BRILLIANT
BLUE).
Gel diffusion may involve SINGLE DIFFUSION or DOUBLE DIFFUSION of the single- or double-DIMENSION type. (See also IMMUNOELECTROPHORESIS and ELEK PLATE.)
gel electrophoresis See ELECTROPHORESIS.
gel filtration (molecular sieving) A method for separating
molecules from a mixture by passing the mixture through
a column of e.g. Sephadex, polyacrylamide, or agarose gel;
molecules are separated primarily according to their size and
shape.
gelatin The product obtained by boiling COLLAGEN. Gelatin is
soluble in water at temperatures above ca. 40 C, and a solution
of concentration >ca. 12% (w/v) forms a gel on cooling below
ca. 2835 C; gels of ca. 412% are used e.g. to test the ability
of certain microorganisms to liquefy (i.e., hydrolyse) gelatin (see
GELATINASE). (See also FRAZIERS MEDIUM.)
gelatinase A GELATIN-hydrolysing enzyme. Gelatin can be
hydrolysed (to soluble oligopeptides) by clostridial COLLAGENASES and by any of a range of extracellular proteolytic enzymes
produced e.g. by various bacteria and fungi. The activity of many
gelatinases requires, or is stimulated by, calcium ions.
Gelbstoff
Collectively, the various dissolved and colloidal
organic substances which occur e.g. in lakes and coastal waters
and which may absorb significant amounts of light particularly
at the blue end of the spectrum.
gemma
gene conversion See RECOMBINATION.
gene dosage The number of copies of a given gene per cell or
nucleus. Increased gene dosage may cause higher levels of gene
product if the gene is not autogenously regulated.
gene-for-gene concept (plant. pathol.) See AVIRULENCE GENE.
gene fusion In genetic engineering: the fusion of two DNA
sequences from different genes to form a hybrid gene (see
FUSION PROTEIN, sense 2). The term is sometimes used synonymously with OPERON FUSION. (See also MUDLAC SYSTEM.)
[Gene fusions (commentary): JB (2000) 182 59355938.]
gene gun A device for inoculating a DNA VACCINE directly into the
epidermis; it bombards the surface with gold particles ( 1 m)
that are coated with the target DNA. [Example of use: Inf.
Immun. (2005) 73 29742985.]
gene library See LIBRARY.
gene therapy Genetic modification of certain cells specifically to
correct an inherited disorder or to treat some infectious diseases;
it has been successful e.g. with adenosine deaminase deficiency
but has apparently caused leukaemia-like illness in one patient
[Nature (2002) 420 116118].
In the ex vivo mode, cells from the patient are modified
in vitro and then re-introduced. For example, in ADENOSINE
DEAMINASE DEFICIENCY the patients stem cells are supplemented
with the normal, wild-type gene before re-introduction; lymphocytes derived from the stem cells can then develop normally.
(In some cases stem cells from a normal (histocompatible) donor
are introduced into the patient.) For selecting stem cells the CD34
marker can be used in immunomagnetic enrichment techniques
(see DYNABEADS). In the in vivo mode, modification takes place
within the patient.
Viruses used as vectors (for carrying genetic material
into cells) include adenoviruses (see ADENOVIRIDAE), adenoassociated viruses (see DEPENDOVIRUS) and certain retroviruses
(RETROVIRIDAE), e.g. lentiviruses. Viral vectors are genetically
modified to be replication-deficient and non-pathogenic; the gene
(etc.) to be introduced into cells is inserted into the viral genome
and enters cells during infection.
Sequences/transgenes can be inserted into various types of
dividing or non-dividing cell e.g. by AAVs (small sequences),
adenoviruses (larger sequences) and lentiviruses.
With some viruses the broad range of host cells is problematic
when specific type(s) of cell are to be targeted. In such cases a
virus can be modified by PSEUDOTYPING e.g. adenovirus type
5 was modified to produce a more specifically targeted vector
[JV (2001) 75 29722981].
In CYSTIC FIBROSIS, respiratory epithelial cells have been
targeted (via an inhaler) by LIPOSOMES containing the normal
gene. [Bioch. J. (2005) 387 115.]
genetic drift
GENETIC CODE: the universal code
First base
(5 end)
Second base
Third base
(3 end)
Phe
Phe
Leu
Leu
Ser
Ser
Ser
Ser
Tyr
Tyr
ochre
amber
Cys
Cys
opal
Trp
U
C
A
G
Leu
Leu
Leu
Leu
Pro
Pro
Pro
Pro
His
His
Gln
Gln
Arg
Arg
Arg
Arg
U
C
A
G
Ile
Ile
Ile
Met
Thr
Thr
Thr
Thr
Asn
Asn
Lys
Lys
Ser
Ser
Arg
Arg
U
C
A
G
Val
Val
Val
Val
Ala
Ala
Ala
Ala
Asp
Asp
Glu
Glu
Gly
Gly
Gly
Gly
U
C
A
G
genetic engineering
advantageous nor disadvantageous to the organism. (cf.
ANTI-
GENIC DRIFT.)
gibberellins
disc or sucker by means of which the parasite is believed to
adhere to the intestinal wall of its host (see also GIARDIASIS).
The cell contains a pair of AXOSTYLES, and one or two deeply
staining, rod- or comma-shaped bodies (median or parabasal
bodies) which occur in the centre of the cell and are orientated
more or less perpendicularly to the long axis of the cell. The
trophozoites reproduce by binary fission; they stain well with
e.g. ironhaematoxylin. [Culture of G. lamblia in serum-free
medium: J. Parasitol. (1983) 69 11811182. Lipid metabolism
in Giardia: TIP (2001) 17 316319.]
G. lamblia forms ovoid cysts (ca. 1115 710 m) in the
gut lumen, and these are expelled with the faeces. Mature cysts
generally contain 4 nuclei which are commonly clustered at one
pole. The nuclei and portions of the median bodies and flagella
can be seen in cysts stained with e.g. iodine.
The classification of Giardia strains into species remains
controversial. Strains are often named according to the host in
which they are found e.g. G. canis (from dogs) but such
speciation may not be justified. It has been proposed that only
three species be recognized on the basis of morphology and
host range: G. agilis (from frogs and tadpoles), G. muris (from
rodents and birds), and G. duodenalis (from mammals); strains
currently known as G. lamblia would thus be included in the
species G. duodenalis.
giardiasis (lambliasis) A human disease caused by Giardia
lamblia. Infection occurs by ingestion of cysts; transmission may
occur by person-to-person contact of via contaminated food or
drinking water (cysts can survive levels of chlorination used for
treating WATER SUPPLIES).
Incubation period: 47 days. Infection may be asymptomatic, or there may be acute or chronic diarrhoea, often with
nausea, weight loss, fatty stools and flatulence. Symptoms are
believed to be due to mechanical obstruction of the intestinal
mucosa; tissue invasion does not occur. Although adhesion of
G. lamblia to the mucosa of the small intestine is generally
believed to depend on the organisms sucker (see GIARDIA),
adhesion may involve a specific giardial LECTIN which is activated by gut proteases [Science (1986) 232 7173].
Diagnosis. Trophozoites may be detected by microscopy in
(fresh) saline-mounted specimens of diarrhoea; cysts, rather than
trophozoites, may be found in specimens of formed stool. An
ELISA-based method, using polyclonal antibodies, may be used
to detect Giardia antigens in faeces.
Chemotherapy: e.g. METRONIDAZOLE, QUINACRINE.
[Giardia in drinking water supplies (cyst levels, parasite
viability, health impact): AEM (1996) 62 4754.]
Gibberella A genus of fungi (order HYPOCREALES) which include
plant-pathogenic species (see e.g. BAKANAE DISEASE); anamorphs
occur in the genus FUSARIUM. Gibberella spp form blue- or
violet-coloured superficial perithecia, and ovoid to fusiform
ascospores. (See also GIBBERELLINS and ZEARALENONE.)
gibberellic acid GIBBERELLIN A3 .
gibberellins A class of PHYTOHORMONES which are synthesized
e.g. in the leaves of plants and which regulate stem elongation,
seed germination, etc; gibberellins were originally discovered as
products of the fungus Gibberella fujikuroi (Fusarium moniliforme). Many gibberellins have now been identified and designated gibberellins A1 , A2 etc (or GA1 , GA2 etc); all share
a common tetracyclic structure, but differ in the position and
nature of their substituents.
The production of gibberellins by G. fujikuroi is believed
to play an important role in the pathogenesis of BAKANAE
DISEASE; another example of a plant pathogen which produces
Gloeocapsa
in a number of bacteria and cyanobacteria. In bacteria of
the CytophagaFlexibacter group, sulphonolipids in the cell
envelope appear to be necessary for gliding motility [Nature
(1986) 324 367369].
In some gliding bacteria certain stages in the life cycle (e.g.
the myxospore in myxobacteria) are non-motile. In Flexibacter
elegans (cells ca. 150 m) gliding occurs only in those cells
which are longer than ca. 5 m.
In some cyanobacteria, motility has been associated with
the junctional pore complex (JPC): a channel in the cell
envelope through which mucilage (carbohydrate) is secreted;
each organism has a number of JPCs, and secretion via these
channels is believed to provide the thrust that is necessary for
locomotion [JB (2000) 182 11911199].
Results of studies on Myxococcus xanthus (involving shockfreezing and freeze-drying) have indicated that the motility
apparatus in this organism resembles a helical continuum
or band (170380 nm wide) that is wrapped around the
protoplast (i.e. within the periplasmic space) to form a closed
loop; nodes, associated with the continuum, may travel along
the trichomes in a wave-like fashion (but with variable internode distance), each node possibly corresponding to a region of
close contact, or adhesion, between the trichome and substratum
[Microbiology (2001) 147 939947].
Gliocladium See HYPHOMYCETES and GLIOTOXIN.
gliotoxin An epidithiapiperazinedione MYCOTOXIN (see EPIPOLYTHIAPIPERAZINEDIONES) obtained from Trichoderma viride and
from species of Aspergillus, Gliocladium and Penicillium; it
inhibits replication of polioviruses, echoviruses and measles
virus, and also has antibacterial, antifungal and antitumour activity. In eukaryotic cells an early effect of gliotoxin is apparently
disruption of microfilaments [JCS (1986) 85 3346].
glmM gene
In Helicobacter pylori : a gene (formerly ureC )
which encodes phosphoglucosamine mutase.
gln genes See e.g. NTR GENES.
global regulatory system Syn. REGULON.
global warming See GREENHOUSE EFFECT.
Globigerina A genus of pelagic foraminifera (order FORAMINIFERIDA). The test is calcareous and multiloculate, the rounded
locules being spirally arranged. G. bulloides may reach ca.
800 m diam., and numerous fine calcareous spines radiate from
the test; G. bulloides and e.g. G. inflata, G. pachyderma and
G. quinqueloba occur in subpolar and cold temperate seas.
Globigerinoides A genus of pelagic foraminifera (order FORAMINIFERIDA). G. sacculifer is often abundant in tropical and subtropical seas, occuring in the upper euphotic zone; it is ca.
0.51.0 mm diam., bears radial spines 12 mm long, and contains numerous zooxanthellae.
globomycin See e.g. BRAUN LIPOPROTEIN.
globose Spherical.
globoside (parvovirus receptor) See ERYTHROVIRUS.
Gloeobacter A genus of unicellular CYANOBACTERIA (section I)
in which the rod-shaped cells divide by equal binary fission
in one plane and occur in colonial aggregates surrounded by
a sheath; the cells are characterized by their lack of THYLAKOIDS photosynthesis and respiration apparently being associated with the cytoplasmic membrane. Phycobiliproteins occur
as an electron-dense layer of characteristically shaped phycobilisomes (apparently composed of bundles of rods) beneath
the cytoplasmic membrane [Arch. Micro. (1981) 129 181189].
GC% (one strain): 64.
Gloeocapsa A genus of unicellular CYANOBACTERIA (section I)
in which the cells are coccoid and divide by equal binary
Glaucoma A genus of ciliates (order HYMENOSTOMATIDA). G. scintillans is ovoid, ca. 4080 m, with uniform somatic ciliature;
it is common in freshwater habitats containing decomposing
organic matter (see also SAPROBITY SYSTEM). G. dragescui also is
ovoid, but G. frontata is elongate with a pointed posterior end.
Glaucophyta A phylum of algae which includes those species
that contain CYANELLES instead of CHLOROPLASTS. The phylum
contains wall-less organisms (e.g. the flagellated, cryptomonadlike Cyanophora) and species which have a cell wall (e.g. Glaucocystis). In Cyanophora the (cyanobacterial) endosymbiont is a
species of Cyanocyta; synthesis of phycocyanin by the endosymbiont is apparently partially dependent on the hosts ribosomes.
glaucous Bluish-green, or covered with a bluish-green powdery
or waxy bloom.
GLC Gasliquid CHROMATOGRAPHY.
GlcNAc N-ACETYL-D-GLUCOSAMINE.
gleba In the fruiting bodies of e.g. fungi of the GASTEROMYCETES:
the spore-bearing tissue which is (at least initially) enclosed by
the PERIDIUM (or by the wall of the peridiole in members of the
NIDULARIALES).
Glenodinium See DINOFLAGELLATES.
gliding bacteria A non-taxonomic group of bacteria and
cyanobacteria which exhibit GLIDING MOTILITY during at least
some stage in their life cycles; gliding bacteria typically
occur in soil and in freshwater and marine habitats. The
group comprises the genera listed under CYTOPHAGALES,
the MYXOBACTERALES, the CHLOROFLEXACEAE, members of
the cyanobacteria both unicellular (e.g. Synechococcus)
and filamentous (e.g. Anabaena, Oscillatoria, Phormidium,
Spirulina) and e.g. Capnocytophaga and Desulfonema.
Although not formally included among the gliding bacteria, some species of Mycoplasma exhibit a form of surfaceassociated locomotion referred to as gliding.
gliding motility A continuous-type (i.e. smooth, non-jerky)
MOTILITY which occurs in some prokaryotes (GLIDING BACTERIA),
algae (e.g. some diatoms and desmids) and protozoa (e.g. Toxoplasma gondii ) which have no obvious locomotory organelles;
gliding motility appears to occur only on a solid surface.
In the diatom Amphora coffeaeformis, some studies have
suggested a possible mechanism that involves actin- and tubulinbased structures; this is compatible with the theory that gliding
results from the translocation of membrane proteins along the
raphe canal the outermost part of such proteins being attached
to the immobile slime secretion which has adhered to the
substratum [Cell Mot. (1985) 5 103122].
In the gregarine Gregarina garnhami (which apparently does
not contain actin) it has been suggested that gliding may involve
two sets of filaments which run longitudinally in the pellicle
[JUR (1984) 88 6676].
Gliding motility has been extensively investigated in prokaryotes [early review: ARM (1981) 35 497529]. In some species,
individual cells glide quite slowly (a few micrometres per
minute) while in other species the cells may achieve speeds
of up to ca. 150 micrometres per minute; some gliding bacteria
can also perform other types of movement (e.g. flexing, twitching see e.g. SPIRULINA). The path of a gliding cell is marked
by a slime trail, and on an agar surface the path may be etched
into the agar; at least some gliding bacteria can penetrate agar
gels. Gliding is also exhibited by trichomes and by aggregates
of cells (swarms).
Typically, gliding bacteria glide when nutrient levels are
low; high levels can suppress gliding. Gliding appears to
require the presence of calcium ions and is inhibited by EGTA
339
Gloeochloris
fission in two or three planes, giving rise to clusters of cells
enclosed in a sheath. GC%: 4046. The organisms grow often
in masses on wet rocks e.g. in the supralittoral zones of rocky
coasts. (cf. GLOEOTHECE.)
Gloeochloris
A genus of algae of the XANTHOPHYCEAE. The
vegetative cells occur in a spherical palmelloid colony; asexual
reproduction occurs by the formation and release of biflagellate
zoospores.
Gloeodinium A genus of DINOFLAGELLATES which form palmelloid colonies and reproduce by zoospore formation. One species
(G. montanum), found in freshwater peaty marshes.
Gloeothece A genus of unicellular CYANOBACTERIA (section I);
the cells are rod-shaped (ca. 56 m wide), possess thylakoids
(cf. GLOEOBACTER), divide by equal binary fission in one plane
(cf. GLOEOCAPSA), and occur in colonial aggregates surrounded
by a well-defined sheath (cf. SYNECHOCOCCUS). The function of
the sheath seems not to include the protection of nitrogenase
from oxygen [oxygen relationships in nitrogen fixation: MR
(1992) 56 346347]. Strains of Gloeothece can carry out NITROGEN FIXATION aerobically, despite the absence of heterocysts, and
were formerly regarded as nitrogen-fixing strains of GLOEOCAPSA.
GC%: 4043.
Gloeotrichia
A phycological genus of the RIVULARIACEAE
(now included in the genus CALOTHRIX). G. echinulata is a
gas-vacuolate, freshwater planktonic species which may form
blooms; in nature, it forms characteristic spherical urchin-like
colonies in which the terminal heterocysts occur in the centre of
the colony and the trichomes radiate outwards. Hair cells may
be formed e.g. under phosphorus-deficient conditions.
Gloiopeltis See RHODOPHYTA.
glomerulonephritis Inflammation of the kidney glomeruli. Acute
glomerulonephritis is characterized by blood and red cell casts in
the urine, and a reduced glomerular filtration rate leading to oliguria, oedema and hypertension. It may be due to deposition in the
glomeruli of antigen-antibody complexes formed during certain
infectious diseases, e.g., SYPHILIS (see also POST-STREPTOCOCCAL
GLOMERULONEPHRITIS); in mice it may be induced e.g. by the
LCM VIRUS. (See also PYELONEPHRITIS.)
Glomospira See FORAMINIFERIDA.
Glomus See ENDOGONALES.
glorin See POLYSPHONDYLIUM.
Glossina (tsetse fly)
A genus (22 species) of haematophagous
(blood-sucking) flies (order Diptera) which include vectors of
salivarian trypanosomes; they occur in sub-Saharan Africa in
a belt approximately 15 N15 S, and in SE Africa, including Mozambique. Glossina spp are distinguished from other
dipterans e.g. by the chopper-shaped hatchet cell in the wing
venation. Both the male and female flies suck blood.
glove box A cabinet, the interior of which is accessible via
gloves attached to openings in the front panel. (See also SAFETY
CABINET.)
glove juice test A test used (in the USA) to determine the efficacy
of a given antimicrobial agent used as a surgical hand scrub
[Book ref. 65, pp. 958961].
GlpF See MIP CHANNEL.
glucan A homoglycan (see POLYSACCHARIDE) consisting of glucose residues see e.g. CELLULOSE, GLYCOGEN, LUTEOSE, NIGERAN, PARAMYLON, STARCH. (See also CELL WALL (fungal).)
glucitol Syn. SORBITOL.
glucoamylases Syn. g-AMYLASES.
glucobrassicin See CLUBROOT.
glucocorticoids Steroid hormones, produced in the adrenal cortex,
whose activity includes regulation of carbohydrate and protein metabolism. Glucocorticoids also have anti-inflammatory
activity; thus, e.g. they inhibit the ability of IFN-g and lipopolysaccharides to induce the synthesis of CYTOKINES in macrophages.
glucogenesis Syn. GLUCONEOGENESIS.
glucomannans See MANNANS.
gluconate See GLUCONIC ACID.
gluconeogenesis (glucogenesis) The synthesis of glucose (and
hence other hexoses) from non-carbohydrate substrates such
as acetate, glycerol, pyruvate, succinate etc. Essentially, this
may be achieved by conversion (where necessary) of the
substrate to an intermediate of the EMBDENMEYERHOFPARNAS
PATHWAY [Appendix I(a)], followed by reversal of reactions of the
EMP pathway the three irreversible reactions in this pathway
being bypassed by other enzymes. Thus, e.g., in Escherichia
coli phosphoenolpyruvate can be synthesized from pyruvate
or from the TCA CYCLE intermediates oxaloacetate and malate
[see Appendix II(b)]; phosphoenolpyruvate is then converted to
fructose 1,6-bisphosphate by reversal of reactions of the EMP
pathway. Fructose 1,6-bisphosphate is hydrolysed by fructose
bisphosphatase to fructose 6-phosphate which can in turn be
converted to glucose 6-phosphate by phosphohexose isomerase.
gluconic acid Gluconic acid and its salts are metabolized by various microorganisms (see e.g. ENTNERDOUDOROFF PATHWAY), and
are synthesized (by the oxidation of glucose) e.g. by Aspergillus
niger and other hyphomycetes and by Gluconobacter oxydans.
A. niger and G. oxydans are used as commercial sources of these
compounds which have a range of uses in the food and pharmaceutical industries; for example, gluconic acid (a chelating
agent) is used for sequestering metal ions; sodium gluconate is
used for cleaning glassware and for removing rust from metals; calcium and iron gluconates are used therapeutically for the
treatment of calcium and iron deficiencies.
Gluconobacter A genus of Gram-type-negative bacteria of the
ACETOBACTERACEAE; the organisms occur e.g. on certain fruits
and flowers, and are used e.g. for the production of MONOBACTAMS and in the SORBOSE FERMENTATION. Cells: typically ovoid
to rod-shaped, 0.50.8 0.94.2 m, non-motile or lophotrichously flagellate. Catalase-positive. Typically, ethanol is oxidized to acetic acid on e.g. CARR MEDIUM; neither acetate nor
lactate is oxidized to CO2 . Ketogenic growth occurs on polyalcohol substrates, and all strains form 2-ketogluconic acid (and
most form 5-ketogluconic acid) from D-glucose. Substrates utilized include e.g. D-mannitol, sorbitol, glycerol (see DIHYDROXYACETONE FERMENTATION), D-fructose and D-glucose; all strains
require growth factors (which may include e.g. pantothenate,
niacin, thiamine, PABA) when D-mannitol is used as the sole
carbon source. The organisms lack a complete TCA cycle; the
breakdown of sugars and polyols to CO2 occurs mainly via the
HEXOSE MONOPHOSPHATE PATHWAY. Optimum growth temperature:
2530 C. GC%: ca. 5664. Type species: G. oxydans which
incorporates strains previously referred to as Acetobacter suboxydans.
glucose dehydrogenase See QUINOPROTEIN and EXTRACYTOPLASMIC OXIDATION.
glucose effect (glucose repression) (1) Syn. CATABOLITE REPRESSION. (2) Syn. CRABTREE EFFECT.
glucose isomerase (xylose isomerase; D-xylose ketolisomerase;
EC 5.3.1.5) An intracellular enzyme which converts D-glucose
to D-fructose, although its main function in vivo is probably the
conversion of D-xylose to D-xylulose; the enzyme is typically
induced in the presence of xylose. Glucose isomerase, obtained
e.g. from Bacillus coagulans (see IMMOBILIZATION (1)) or
Streptomyces spp, is used commercially on a large scale for the
340
glycocalyx
conversion of D-glucose to D-fructose e.g. in the manufacture of
HIGH-FRUCTOSE CORN SYRUP. (See also ENZYMES.)
glucose oxidase (b-D-glucose:oxygen 1-oxidoreductase, EC 1.1.3.4)
An enzyme (produced e.g. by Aspergillus and Penicillium spp)
which oxidizes glucopyranose in the presence of oxygen to Dglucono-d-lactone and H2 O2 the former rapidly hydrolysing to
D-gluconic acid. Glucose oxidase from e.g. Aspergillus niger (a
glycoprotein containing 2FAD/molecule) is widely used in clinical tests for the detection of glucose in urine, blood etc; in general,
such tests rely on a colour change resulting from the oxidation of a
chromogen by H2 O2 released by glucose oxidase in the presence
of glucose and oxygen. Glucose oxidase is also used in the food
industry e.g. for removing glucose from foods (e.g. eggs preparatory to drying) to prevent browning, and for removing oxygen
from e.g. beer, wine, mayonnaise etc. (See also ENZYMES.)
b-glucosidase See CELLULASES.
b-glucoside permease (in Escherichia coli ) See CATABOLITE REPRESSION.
glucosinolase See CLUBROOT.
Glugea
A genus of protozoa (class MICROSPOREA) which are
parasitic in fish; tumour-like cysts (XENOMAS, glugea cysts)
ca. 24 mm diam. develop in the gut mucosa and liver of the
infected fish.
glume blotch A CEREAL DISEASE, caused by Leptosphaeria nodorum (Septoria nodorum), which can affect e.g. wheat and barley.
Leaf lesions are initially yellow, later becoming golden-brown
and sometimes coalescing. Lesions on glumes (usually spreading
from the tip) are a dark purplish-brown, and they later exhibit
dark or black pycnidia. Control: e.g. CARBENDAZIM or PROCHLORAZ with a DITHIOCARBAMATE.
L-glutamate See GLUTAMIC ACID.
glutamate dehydrogenase See AMMONIA ASSIMILATION.
glutamate synthase See AMMONIA ASSIMILATION.
L-glutamic acid An amino acid synthesized by the reductive
amination of 2-oxoglutarate see Appendix IV(a). It is produced commercially on a large scale for use in the food
industry mainly as a flavour enhancer (monosodium glutamate) and is obtained from strains of bacteria (e.g. Corynebacterium glutamicum, glutamic acid bacteria) grown aerobically
on e.g. molasses or starch hydrolysates. (Some strains can be
grown e.g. on acetic acid.) The strains used require biotin for
growth and have little or no 2-oxoglutarate dehydrogenase activity (so that metabolism of 2-oxoglutarate via the TCA cycle is
limited or cannot occur). Production of glutamic acid is maximal
under suboptimal growth conditions (achieved e.g. by limiting
biotin). The glutamic acid must be secreted by the cells to avoid
feedback inhibition of its synthesis; permeability of the cells
may be increased e.g. by biotin deficiency, by treatment with
fatty acid derivatives or antibiotics (e.g. penicillin), or by using
strains auxotrophic for glycerol or oleic acid grown on low levels
of glycerol and oleic acid, respectively.
Some L-glutamine is also formed during glutamic acid production; the proportion of glutamine formed can be increased by
adjusting conditions of pH, nutrient availability etc.
L-glutamine An amino acid synthesized from GLUTAMIC ACID:
see Appendix IV(a). It is an important intermediate in various
metabolic pathways, being involved e.g. in some types of AMMONIA ASSIMILATION and in various transamination reactions e.g.
in the biosynthesis of tryptophan and of purine nucleotides [see
Appendixes IV(f) and V(a)].
glutamine synthetase See AMMONIA ASSIMILATION.
glutaraldehyde (CHO(CH2 )3 CHO) A dialdehyde whose two
aldehyde groups can substitute amino and other groups in proteins and nucleic acids and which can thus form cross-links in
glycocholic acids
glyoxysome A type of MICROBODY which occurs in plant cells,
and in some eukaryotic microorganisms, and which contains
enzymes of the glyoxylate cycle.
glypiated protein A protein which is anchored to a component
of the eukaryotic cell membrane (glycosylphosphatidylinositol)
via a carbohydrate chain (to which the protein is attached).
Gm allotype See ALLOTYPE.
GM-CSF See COLONY-STIMULATING FACTORS.
GM gangliosides See SPHINGOLIPID.
GMP Guanosine 5 -monophosphate: see Appendix V(a).
GMS Gomori METHENAMINESILVER STAIN.
GN broth Gram-negative enrichment broth (used e.g. for the
enrichment of shigellae from food or faeces); it contains enzymic
digest of casein and animal tissue, D-glucose, citrate, deoxycholate,
NaCl, phosphate buffer (pH 7.0). [Recipe: Book ref. 47, p. 652.]
Gnomonia See DIAPORTHALES.
gnotobiotic Refers to a microbiologically monitored environment
or animal, i.e., one in which the identities of all microorganisms
present are known. (cf. SPECIFIC PATHOGEN FREE.)
goat pox A goat disease, clinically similar to SHEEP POX, caused
by a Capripoxvirus which is antigenically distinguishable from
the sheep pox virus.
GOGAT See AMMONIA ASSIMILATION.
gold leaching See LEACHING.
gold standard (lab. microbiol.) Any well-established procedure
(e.g. a diagnostic test) which is generally regarded as the superior
and definitive method, and which is used as a reference against
which other, proposed or alternative methods may be compared
(often in terms of sensitivity and/or specificity).
In many cases culture is regarded as the gold standard for
diagnostic purposes. However, with the advent of nucleic-acidbased methods, some authors refer to an expanded or combined
gold standard; using such a standard, a true-positive result is one
that is positive by the gold standard method (usually culture)
and by one nucleic-acid-amplification test [example of use of
the term expanded /combined gold standard: JCM (1997) 35
957959].
For diagnostic tests on Chlamydia trachomatis, some authors
have used an aggregate gold standard in which a sample is
deemed to give a true-positive result if it is either culture-positive
or positive in two non-culture assays.
GoldbergHogness box See PROMOTER.
golden algae CHRYSOPHYTES.
Golgi apparatus An intracellular organelle consisting typically
of a number of stacks of flattened membranous vesicles (cisternae); at least one Golgi apparatus occurs in most types of
eukaryotic cell (cf. e.g. DIPLOMONADIDA). Within the cell the
Golgi apparatus is characteristically orientated such that one
end of the stacked cisternae (the proximal or forming end)
is nearer the nucleus; the opposite end is called the distal or
maturing end. Functions of the Golgi apparatus include the
formation of LYSOSOMES and the formation of secretory vesicles
within which e.g. macromolecules or cell envelope substructures
can be transported to the cell surface (see e.g. PALADE PATHWAY
and CELL WALL (a)). Secretory molecules reach the Golgi apparatus primarily from the ENDOPLASMIC RETICULUM; thus, e.g., a
portion of smooth ER forms a vesicle which encloses molecules
from the lumen of the ER, and the vesicle passes through the
cytoplasm and fuses with a similar vesicle or with a cisterna
at the forming end of the Golgi apparatus. Presumably as a
result of repeated budding and fusion, the contents of a vesicle eventually reach the maturing end of the Golgi apparatus and are finally enclosed within a secretory vesicle which
gradostat
fuses with the cytoplasmic membrane. During transit through
the Golgi apparatus a molecule characteristically increases its
degree of glycosylation fucose, galactose and/or neuraminic
acid residues typically being added.
(See also DICTYOSOME.)
Gomori stain Syn. METHENAMINESILVER STAIN.
Gomphonema A genus of pennate DIATOMS. In e.g. G. olivaceum
the cell adheres to the substratum by a stalk of secreted
mucilage.
gonal nucleus See CONJUGATION (1)(c).
Gonapodya See MONOBLEPHARIDALES.
Gonatobotrys See HYPHOMYCETES and CONIDIUM.
Gonatobotryum See HYPHOMYCETES.
gongylidia (sing. gongylidius) Nodular fungal structures which
develop in the FUNGUS GARDENS of parasol ants or in the fungus
combs of termites (see TERMITEMICROBE ASSOCIATIONS).
gonidium A cell which is involved in asexual reproduction: see
e.g. LEUCOTHRIX and VOLVOX. (The term was once applied to a
photobiont cell in a lichen in the mistaken belief that such cells
served a reproductive function.)
Gonimochaete See ENTOMOPHTHORALES.
gonococcal ophthalmia See GONORRHOEA.
gonococcus Neisseria gonorrhoeae.
Gonometa virus See PICORNAVIRIDAE.
gonorrhoea (gonorrhea) An acute or chronic VENEREAL DISEASE
which in nature affects only man; it is caused by Neisseria
gonorrhoeae (the gonococcus see NEISSERIA). Incubation
period: 25 days or longer. Gonococci adhere to the urethral
epithelium by means of fimbriae; they penetrate the mucosa,
causing an acute inflammatory response, and the infection
spreads readily to adjacent tissues. In males, infection may
be asymptomatic or may involve URETHRITIS, with painful
urination and a yellowish mucopurulent discharge; prostatitis
and epididymitis may occur. In females, infection may be
asymptomatic or there may be a purulent vaginal discharge;
infection may spread via the endometrium, fallopian tubes and
ovaries to the pelvic peritoneum (pelvic inflammatory disease,
PID). (See also CURTISFITZ-HUGH SYNDROME.) In either sex,
sterility may result. Some strains of gonococci may become
disseminated: bacteraemia, associated with e.g. fever, may
be followed by skin lesions, arthritis, and (sometimes fatal)
endocarditis and/or meningitis. Gonococcal contamination of the
eyes may lead to conjunctivitis (gonococcal ophthalmia) which
can cause blindness if untreated; infants may be infected during
birth (ophthalmia neonatorum), and neonates may therefore be
prophylactically treated with eye-drops containing e.g. 1% w/v
silver nitrate (Crede procedure) or penicillin. Lab. diagnosis:
smears of the discharge are stained (e.g. by the Gram stain
or fluorescent antibody techniques) to reveal large numbers of
diplococci in PMNs. Culture (e.g. on THAYERMARTIN AGAR)
may be necessary, especially for diagnosing females. A PROBEbased test (the PACE 2C test) has been used for detecting
N. gonorrhoeae and Chlamydia trachomatis in a single assay
(particularly useful because co-infection with these two pathogens
is quite common) [evaluation of the PACE 2C test with
endocervical specimens: JCM (1995) 33 25872591]. A test
for detecting N. gonorrhoeae based on the ligase chain reaction
(see LCR) reported results superior to those obtained by culture
[JCM (1997) 35 239242].
Chemotherapy depends on (changing) patterns of antibiotic
resistance in the pathogen; penicillins (with probenecid), tetracycline, erythromycin and spectinomycin have been used.
Gonyaulax See DINOFLAGELLATES; BIOLUMINESCENCE; RED TIDE.
GraffReinet disease
to the lower permeability of their cell walls: the PEPTIDOGLYCAN
of Gram-positive cell walls is more extensively cross-linked
than that in Gram-negative species. (N.B. Mammalian cells are
uniformly Gram-negative.)
The cells of some bacteria (e.g. Bacillus spp) are strongly
Gram-positive when young, but tend to become Gram-negative
in ageing cultures; this may reflect degenerative changes in the
cell wall. Some bacteria give a Gram-variable reaction, i.e.,
they are sometimes Gram-positive, sometimes Gram-negative;
this could reflect e.g. minor variations in staining technique. To
avoid the taxonomic problems of Gram-variable bacteria it has
been suggested that classification be based on GRAM TYPE rather
than on GRAM REACTION.
Gram type A taxonomically useful designation (either Gram
type positive or Gram type negative) which is based on biochemical and anatomical properties of a bacterial cell (see e.g.
CELL WALL) rather than on GRAM REACTION; designation on this
basis avoids the taxonomic problems caused by a Gram-variable
reaction in the GRAM STAIN. [JGM (1982) 128 22612270.]
Gram-variable See GRAM STAIN.
gramicidins A group of linear peptide ANTIBIOTICS, each of
which has a formyl group at the N-terminal and an ethanolamine
residue at the C-terminal. (Gramicidin J, also called gramicidin S, is misnamed: it is a TYROCIDIN.) Gramicidins act as
channel-forming IONOPHORES, forming transient ion-conducting
dimers in lipid bilayers; such channels permit the passage of a
range of hydrated monovalent cations as well as protons. Against
Gram-positive bacteria gramicidins may be bacteriostatic or (at
higher concentrations) bactericidal; most Gram-negative bacteria
tend to be resistant.
grana See CHLOROPLAST.
granulin See BACULOVIRIDAE.
granulocyte See PMN.
granuloma A type of lesion resulting from a local inflammatory
response to a persistent antigen or toxin at a given site in the
body; the lesion consists of a hard mass composed mainly of
macrophages and strands of fibrous connective tissue although
other types of cell (e.g. lymphocytes, plasma cells, polymorphs
etc) may also be present, and the lesion may also contain
GIANT CELLS. Granuloma formation involves a T cell-dependent
immune response. (See also DELAYED HYPERSENSITIVITY.)
granuloma inguinale (donovanosis) A chronic human disease,
occuring mainly in the tropics and subtropics, in which granulomatous ulcers develop chiefly on the genitals; the causal agent,
Calymmatobacterium granulomatis, is transmitted by intimate
contact. In smears (stained e.g. with Wrights stain) the pathogen
appears as clusters of blue or black Donovan bodies in the
cytoplasm of large mononuclear cells.
granuloplasm See e.g. SARCODINA.
Granuloreticulosea A class of protozoa (superclass RHIZOPODA)
which form delicate, finely granular or hyaline reticulopodia
(or, rarely, finely pointed, granular, non-anastomosing pseudopodia). Orders: Athalamida (amoebae naked: e.g., Arachnula,
Biomyxa); Monothalamida (amoebae enclosed in a singlechambered organic or calcareous test, not exhibiting an alternation of generations: e.g., Lieberkuehnia); FORAMINIFERIDA.
granulose (1) (noun) A (1 4)-a-glucan which accumulates in
the cells of Clostridium spp prior to sporulation; it is rapidly
degraded during sporulation, and may thus function as an
endogenous reserve of carbon and energy for sporulation.
(2) (adj.) Having a granular appearance.
granulosis An INSECT DISEASE caused by a GRANULOSIS VIRUS.
granulosis viruses (GVs) Viruses belonging to subgroup B of
the BACULOVIRIDAE (q.v.). The viruses replicate mainly in the
gregarine movement
green spot disease See ALGAL DISEASES.
green sulphur See SULPHUR.
green sulphur bacteria See GREEN BACTERIA.
GreenbergSmith sampler An ALL-GLASS IMPINGER.
greenhouse effect The warming of the planet due to rising levels
of CO2 , methane and certain other gases (which effectively trap
some of the radiant energy reaching the Earths surface).
In the CARBON CYCLE, large amounts of CO2 are produced by
animals, plants and microbes during respiration or fermentation,
but large amounts are used (fixed) during PHOTOSYNTHESIS;
globally, the important balance between biological production
and uptake of CO2 is being upset e.g. by the burning of
vast amounts of fossil fuel (gas, petroleum etc.). (See also
METHANOTROPHY.)
It might be thought that raised levels of CO2 would stimulate
growth in plants, and, thereby due to greater sequestration of
CO2 by photosynthesis tend to offset the rise in CO2 . Some
agricultural, crop-type plants do respond to increased CO2 by
improved growth. However, experimental tropical ecosystems
under increased CO2 have shown, in addition to increased root
growth, an increased efflux of CO2 from soil to atmosphere; this
efflux was apparently due to stimulated metabolic activity of
microorganisms in the RHIZOSPHERE. Thus, an increased uptake
of CO2 by plants may itself be offset by increased efflux of CO2
from the soil [Science (1992) 257 16721675].
More recently it was suggested that certain pasture grasses in
the South American savannas may offer a useful sink for carbon
in their particularly massive and deep root systems [Nature
(1994) 371 236238].
It has been pointed out that global warming may itself result
in increased levels of greenhouse gases i.e. a potential positive
feedback effect [BC (1996) 5 10691083].
It has been assumed that the avoidance of deforestation is
of major importance in the context of global warming because
such a policy preserves a valuable means for controlling levels of
atmospheric carbon dioxide [Nature (2001) 410 429]. However,
recent experiments have indicated that the ability of forest
systems to sequester carbon dioxide may be limited by shortages
of nutrients and water and/or by the relatively rapid turnover of
organic carbon in the litter layer [Nature (2001) 411 469472;
Nature (2001) 411 466469; commentary: Nature (2001) 411
431433].
greening (1) See HAEMOLYSIS. (2) See MEAT SPOILAGE and DFD
MEAT.
gregarin The trophozoite form of a gregarine.
Gregarina A genus of the GREGARINASINA.
Gregarinasina (Gregarinidia) A subclass of protozoa (class
SPOROZOASIDA) parasitic in invertebrates (e.g. annelids, insects).
In members of this subclass the mature gametocytes occur
extracellularly in the host (cf. COCCIDIASINA); the mature organism generally has a MUCRON or an EPIMERITE. In the cephaline gregarines (e.g. Gregarina spp) the mature organism is
septate the nucleus usually being in the DEUTOMERITE; in
acephaline gregarines (e.g. MONOCYSTIS) the mature organism
is aseptate. Species whose life cycles do not include schizogony
(the eugregarines) are commonly non-pathogenic; species which
undergo schizogony as well as sexual reproduction (the schizogregarines) are commonly pathogenic. Some authors divide the
schizogregarines into the archigregarines (parasitic in annelids)
and the neogregarines (parasitic in insects). Genera include
Actinocephalus, Stenophora, Urospora.
gregarine A member of the GREGARINASINA.
gregarine movement See MOTILITY.
Gregarinia
Gregarinia (1) A subclass of protozoa (class Telosporea) later
classified as the subclass GREGARINASINA. (2) A subclass of
protozoa (class Sporozoea [JP (1980) 27 3758]) equivalent to
the GREGARINASINA.
Gregarinidia Syn. GREGARINASINA.
grepafloxacin See QUINOLONE ANTIBIOTICS.
grex See DICTYOSTELIUM.
grey mould (botrytis) A disease, caused by Botrytis cinerea,
which can affect a wide range of plants as well as stored fruits
and vegetables (e.g. beans, peas, raspberries and strawberries);
the disease is encouraged by cool, damp conditions, and is
characterized by a grey, fluffy surface mould overlying a soft,
commonly brown, rot. (See also DAMPING OFF.)
grid See ELECTRON MICROSCOPY (a).
Gridley fungus stain A staining procedure that depends on the
oxidation (by chromic acid) of adjacent hydroxyl groups in
fungal cell wall polysaccharides, followed by the reaction of the
resulting aldehyde groups with e.g. SCHIFFS REAGENT. [Method:
Book ref. 53, p. 2207.]
Griffiths tube An apparatus used for grinding tissues. It consists
of a stout, large-diameter glass tube which is closed at the
bottom; the lower, inner part of the tube has a roughened
surface against which the tissue is ground by means of a closefitting pestle-like glass rod.
Griffiths typing (of group A streptococci) A serological (slide
agglutination) TYPING method based on strain differences in the
M and/or T antigens.
Griffithsia See RHODOPHYTA.
Grifola See APHYLLOPHORALES (Polyporaceae).
grippe Syn. INFLUENZA.
griseofulvin (7-chloro-4,6-dimethoxycoumaran-3-one-2-spiro-1 (2 -methoxy-6 -methylcyclohex-2 -en-4 -one)) An antifungal
ANTIBIOTIC produced by Penicillium griseofulvum. It is inhibitory
for actively growing dermatophytes and certain other filamentous
fungi but is inactive against e.g. yeasts and bacteria. Griseofulvin
acts primarily as a MICROTUBULE inhibitor, preventing the assembly of tubulin dimers into microtubules and thereby inhibiting
e.g. mitosis. Additionally, the antibiotic interferes with the pattern of glucan and glycoprotein deposition in the fungal cell
wall; as a result the tips of the hyphae become characteristically
curled (hence the early name for the antibiotic: curling factor).
Griseofulvin is widely used in the treatment of dermatophyte
infections of the skin, hair and nails. It is administered orally
(it is not effective topically) and accumulates in keratinized
tissues; it apparently forms a complex with keratin which may
decrease the susceptibility of the keratin to fungal keratinases.
Griseofulvin-resistant dermatophytes occur [Arch. Derm. (1981)
117 1619].
Griseofulvin is active against certain plant-pathogenic fungi
(e.g. Botrytis spp, Alternaria solani ). It can be taken up by plant
roots and has low phytotoxicity; it has limited use as a systemic
ANTIFUNGAL AGENT in plants.
griseoviridin An antibiotic structurally related to streptogramin
A (see STREPTOGRAMINS).
gRNAs See RNA EDITING.
GrocottGomori stain Syn. METHENAMINESILVER STAIN.
groEL gene See HEAT-SHOCK PROTEINS.
groES gene See HEAT-SHOCK PROTEINS.
Gromia See FILOSEA.
Gromiida See FILOSEA.
groove (in DNA) See DNA.
Grossglockneria See CILIOPHORA.
ground squirrel hepatitis virus (GSHV; ground squirrel hepatitis
B virus, GSHBV) A virus of the HEPADNAVIRIDAE which infects
GSHV
(since each unit on the log2 scale is equal to one generation),
and the graph also indicates clearly any changes in the growth
rate. (The log2 and log10 of any number can be interconverted
by use of the formula: log10 N = 0.301 log2 N.)
The rate of growth may be expressed in terms of the
SPECIFIC GROWTH RATE, m. When m is constant (e.g. during
exponential growth in batch culture), the relationship between m
and the doubling time (i.e. the time taken for the biomass or
population to double) is given by:
td =
0.693
m
(log2 Nt log2 N0 )
t
GSP
GV GRANULOSIS VIRUS.
Gy See GRAY.
Gyalecta See GYALECTALES.
Gyalectales An order of mainly lichenized fungi of the ASCOMYCOTINA. Ascocarp: APOTHECIOID; hamathecium: paraphyses.
Asci: clavate or cylindrical. Genera: e.g. Dimerella, Gyalecta,
Petractis.
GYC agar See ACETOBACTER.
Gymnamoebia A subclass of naked (non-testate) amoebae
(AMOEBIDA, PELOBIONTIDA and SCHIZOPYRENIDA). (cf. TESTACEALOBOSIA.)
Gymnoascales An order of mainly keratinophilic fungi of the
subdivision ASCOMYCOTINA; many species have anamorphs
among the DERMATOPHYTES. Ascocarp: cleistothecioid, with or
without appendages, sometimes insubstantial (consisting e.g.
of a loose hyphal network); sessile or stipitate. Asci: unitunicate. Ascospores: unicellular, spherical, discoid or fusiform,
sometimes forming a mazaedial mass at maturity. Genera: e.g.
AJELLOMYCES, Aphanoascus, ARTHRODERMA, Gymnoascus, Myxotrichum, NANNIZZIA and Onygena (see also MAZAEDIUM); of
these, Aphanoascus and Onygena belong in the family Onygenaceae, and the others in the family Gymnoascaceae.
Gymnoascus See GYMNOASCALES.
gymnocarpic development (also: gymnocarpous development)
(mycol.) The mode of development of a fruiting body in which
the spores are exposed to the environment throughout their
differentiation and maturation. (See e.g. APHYLLOPHORALES; cf.
ANGIOCARPIC DEVELOPMENT.)
Gymnodinioides See HYPOSTOMATIA.
Gymnodinium See DINOFLAGELLATES; RED TIDE; ZOOXANTHELLAE.
Gymnomyxa A protistan phylum (equivalent to the mycological
division MYXOMYCOTA) comprising the subphyla MYCETOZOA,
Plasmodiophorina (equivalent to PLASMODIOPHOROMYCETES), and
Labyrinthulina (equivalent to LABYRINTHULOMYCETES). [Book
ref. 147, pp. 45.]
Gymnosphaera See CENTROHELIDA.
Gymnosporangium
A genus of typically heteroxenous rust
fungi (class UREDINIOMYCETES) whose primary and secondary
hosts are commonly members of the families Juniperaceae and
Rosaceae, respectively. Most species are DEMICYCLIC RUSTS. The
aecial and telial stages often form on GALLS which develop
on the host plant as a response to infection by the rust;
thus, e.g. G. juniperi-virginianae, which parasitizes the juniper
(Juniperus) and apple (Malus), produces telia which develop in
(and later project from) spherical galls (cedar apples) which
form on the juniper. (The cedar (Cedrus) is not susceptible to
this rust.)
Gymnostomatia A subclass of ciliates (class KINETOFRAGMINOPHOREA) in which the cytostome is superficial (i.e., it does
not occur at the base of an organized buccal cavity or vestibulum), and the cytopharyngeal apparatus is of the RHABDOS type.
Somatic ciliature is commonly uniform. The organisms are typically large and carnivorous. Genera include e.g. Acaryophrya,
Acineria, ACTINOBOLINA, COLEPS, Didesmis, DIDINIUM, DILEPTUS,
Holophrya, Lacrymaria, KENTROPHOROS, LOXODES, Loxophyllum, Mesodinium, Metacystis, Nanophrya, PRORODON, STEPHANOPOGON, TRACHELOPHYLLUM and Urotricha.
(See also KARYORELICTID GYMNOSTOMES; PRIMOCILIATID GYMNOSTOMES.)
gymnostome A ciliate of the GYMNOSTOMATIA.
gyrA, gyrB genes See GYRASE.
gyrase (DNA gyrase) A type II TOPOISOMERASE which catalyses
the negative supercoiling of relaxed or positively supercoiled
Gyrosigma
ds cccDNA (see DNA) in an ATP-dependent process. (In the
absence of ATP, the gyrase from Escherichia coli can relax
negative, but not positive, supercoils.) Gyrase functions as a
tetramer consisting of two of each of two types of subunit, A
and B (i.e. A2 B2 ); subunits A and B are the products of genes
gyrA (= nalA) and gyrB (= cou), respectively. The enzyme
binds to dsDNA at specific (but apparently non-homologous)
sites. The DNA becomes wrapped around the surface of the
enzyme in a positive supercoil; this necessarily introduces a
compensating negative supercoil elsewhere in the molecule.
The remaining steps effectively remove the positive supercoil.
The B subunits bind ATP, a step which alters the functional
(conformational?) state of the enzyme, and the A subunits bring
about a staggered break in the dsDNA, the resulting 5 ends
each projecting beyond the 3 ends by four bases. [Determinants
of site-specific DNA breakage by gyrase: EMBO (1986) 5
14111418.] Each 5 end is covalently bound to one of the
A subunits via a phosphotyrosine bond; this allows conservation
of the energy of the phosphodiester bond for later use in resealing. A length of DNA from elsewhere in the molecule
(possibly from the region wrapped around the enzyme) is passed
through the (double-stranded) break while both ends of the
break are held so that they cannot rotate; the break is then resealed. This decreases the linking number of the molecule by
two. (If the translocated length of DNA belongs to a second
molecule, rather than to another part of the same molecule,
the result is a CATENANE.) Finally, the ATP bound to the B
subunits is hydrolysed and the original conformation of the
enzyme is restored; the whole cycle can then begin again.
(Note: ATP binding allows a single round of supercoiling,
but ATP hydrolysis is necessary for subsequent rounds.) The
349
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
H
H Histidine (see AMINO ACIDS).
H antigens Bacterial flagellar antigens. H antigens are detected in
the serological characterization of certain enterobacteria (see e.g.
KAUFFMANNWHITE CLASSIFICATION). Agglutination of cells with
homologous H antiserum occurs rapidly, is characteristically
floccular, and the agglutinated cells can be readily dispersed by
shaking (since flagella are easily broken). H antigens are heatlabile and are destroyed by alcohol but not by dilute formalin.
(See also IMMOBILIZATION TEST.)
In a few Salmonella serotypes (e.g. S. typhi ) and other
enterobacteria the flagella exhibit only one type of antigenic
pattern, i.e. the H antigens are monophasic. However, most
salmonellae can produce either of two different patterns of H
antigens, i.e. in these organisms the H antigens are diphasic
(see PHASE VARIATION).
H+ -ATPase See PROTON ATPASE.
H+ /2e ratio During the operation of an ELECTRON TRANSPORT
CHAIN: the number of protons translocated across the membrane
during the passage of two electrons along the chain.
H-lysin See FURUNCULOSIS (sense 1).
h mutant HOST-RANGE MUTANT.
H+ /O ratio During the operation of an ELECTRON TRANSPORT
CHAIN with oxygen as terminal electron acceptor: the number
of protons translocated across the membrane per oxygen atom
reduced. (cf. P/O RATIO.)
H+ /P ratio The number of protons passing through a PROTON
ATPASE per molecule of ATP released at the catalytic site.
H+ -PPase PROTON PPASE.
H strand Heavy strand: that strand of a dsDNA molecule
which exhibits the higher buoyant density (owing to a higher
content of thymine and guanine) when the dsDNA is denatured
and subjected to CsCl density gradient CENTRIFUGATION; the
other (light) strand is designated the L strand. The designation
heavy or H is also used to refer to a strand labelled with
a heavy isotope such as 15 N, the unlabelled strand being
designated light or L.
H1 protein Syn. H-NS PROTEIN.
H-1 virus See PARVOVIRUS.
HII phase See CYTOPLASMIC MEMBRANE.
HAA See HEPATITIS B VIRUS.
HAART Highly active antiretroviral therapy: a form of chemotherapy, used for HIV-positive and AIDS patients, involving a
combination of different kinds of ANTIRETROVIRAL AGENT; such
treatment should, theoretically, inhibit completely the replication
of HIV, and in some studies HIV is reported to be undetectable in
plasma.
One example of HAART is the combination of (i) efavirenz
(a non-nucleoside reverse transcriptase inhibitor), (ii) nelfinavir
(a protease inhibitor) and (iii) a nucleoside reverse transcriptase
inhibitor [NEJM (1999) 341 18741881].
Even with effective HAART, low-level replication can occur.
This may involve (i) long-lived HIV-infected cells and (ii)
selection of drug-resistant mutants [JV (2005) 79 96259634].
HaberWeiss reaction See HYDROXYL RADICAL.
HACCP Hazard analysis critical control point system: detailed
appraisal of a production process and control of known/potential
hazards at certain critical points in the process. (Hazard refers
to any influence or factor which would, unless avoided, affect
haemolysin
Spontaneous elution (e.g. of influenza viruses) can be inhibited by carrying out haemagglutination tests at 4 C. (c) Passive
haemagglutination: see PASSIVE AGGLUTINATION. (d) The action
of certain LECTINS. (e) Combination between RBCs and bacterial
fimbrial haemagglutinins (see FIMBRIAE).
haemagglutination-inhibition test (HAI or HI test) Any test in
which specific antibody or antigen is detected or quantified
by its ability to inhibit HAEMAGGLUTINATION. HI tests are used
e.g. as clinical diagnostic tests to detect serum antibodies to
haemagglutinating viruses (e.g. influenza and rubella viruses);
essentially, such tests determine the ability of a patients serum
to neutralize the haemagglutinating properties of a suspension of
the given virus neutralization (a positive test) being indicated
by the failure of the serumvirus mixture to agglutinate added
RBCs. In many cases the serum used in such tests must be
pre-treated to (i) abolish its ability to inhibit haemagglutination
non-specifically, and/or (ii) to abolish its ability to promote
haemagglutination. For example, serum may be pre-absorbed
with kaolin (to sequester certain non-specific inhibitors of
haemagglutination) and/or pre-treated with RBCs (of the type
used in the test) in order to absorb HETEROPHIL ANTIBODIES; serum
used in HI tests for e.g. influenza viruses is pre-treated with e.g.
the enzyme RDE, and is then heated (prior to the test) in order
to destroy RDE activity. [Book ref. 53, pp. 20342048.]
HI tests for soluble antigens may involve inhibition of passive
haemagglutination (see PASSIVE AGGLUTINATION) antigen being
preabsorbed to RBCs. Thus, the amount of antigen in a sample
can be measured by the amount of homologous antibody it
can complex (sequester) when mixed with a fixed volume of
antibody; the amount of free (uncombined) antibody remaining
in the mixture (an indirect measure of antigen) is determined by
the addition of antigen-coated RBCs (see BOYDEN PROCEDURE.)
To ensure antigen-specificity in the test, the antiserum should be
preabsorbed with (non-coated) RBCs of the type used in the test.
haemagglutinin Any agent or substance which can bring about
HAEMAGGLUTINATION.
Haemamoeba A subgenus of PLASMODIUM.
haematein A red amphoteric DYE prepared by atmospheric oxidation of an aqueous solution of the colourless compound haematoxylin; haematein is usually referred to as haematoxylin.
haematin Protoporphyrin IXFe(III) hydroxide. (cf. HAEMIN.)
haematogenous (hematogenous) Produced by or derived from
the blood, or disseminated via the bloodstream.
haematophagous Feeding on blood.
haematotropic Syn. HAEMOTROPIC.
haematoxylin See HAEMATEIN.
haematuria The presence of blood in the urine.
haemin (1) Any protoporphyin IXferric iron complex: cf. HAEM
sense 2. (2) Specifically: protoporphyrin IXFe(III) chloride.
(cf. HAEMATIN.)
Haemobartonella A genus of Gram-negative bacteria of the family ANAPLASMATACEAE. Cells: cocci, coccobacilli or rods (range
0.11.5 m) which occur tightly bound to, or within, erythrocytes in the infected host. Haemobartonella spp (H. canis,
H. felis and H. muris) have a wide host range and occur worldwide; they are transmitted e.g. by biting insects.
haemocytometer See COUNTING CHAMBER.
haemoglobinuria The presence of free haemoglobin in the urine.
Haemogregarina See ADELEORINA.
haemogregarines An imprecise name for those protozoa of the
suborders ADELEORINA and EIMERIORINA which infect red and/or
white blood cells in the vertebrate host.
haemolysin (1) Any antibody homologous to the surface antigens of red blood cells (RBCs). (See also IMMUNE HAEMOLYSIS.)
haemolysis
(2) (Syn. haemolytic toxin) Any of various microbial products
which cause HAEMOLYSIS by damaging the cytoplasmic membrane of RBCs.
(a) Aeromonas salmonicida haemolysins. See e.g. FURUNCULOSIS (H-lysin and T-lysin).
(b) Bacillus haemolysins. See e.g. SURFACTIN.
(c) Clostridium haemolysins. See CLOSTRIDIUM.
(d) Escherichia coli haemolysins.
a-Haemolysin is an extracellular haemolysin (MWt ca.
107000) specified by either chromosomal or plasmid-borne
genes (hly genes); chromosomal and plasmid-borne hly genes
are closely homologous, and identical hly genes can occur
on plasmids of different incompatibility groups. In cultures of
E. coli, production of a-haemolysin occurs under aerobic and
anerobic conditions, but is enhanced by aerobiosis and inhibited by >100 M iron. a-Haemolysin can lyse the RBCs of e.g.
sheep, rabbits and man causing clear haemolysis on blood agar
plates; it is cytotoxic for human leucocytes and is lethal when
injected into mice. a-Haemolysin appears to insert into lipid
bilayers, generating hydrophilic transmembrane pores of effective diameter ca. 3 nm [Inf. Immun. (1986) 52 6369]. [Review:
MR (1984) 48 326343; role of a-haemolysin in the pathogenesis of experimental E. coli infection in mice: JGM (1985) 131
395403.]
b-Haemolysin is a cell-bound haemolysin active against e.g.
rabbit and human RBCs; it causes clear haemolysis on blood
agar plates.
g-Haemolysin has been reported in nalidixic acid-resistant
E. coli mutants, and its production is stimulated by nalidixic
acid; it is not lytic for human or rabbit RBCs.
(e) Staphylococcus haemolysins are produced by both coagulase-positive and -negative strains; the best known are the protein
EXOTOXINS a-, b-, g- and d-haemolysins, although others also
occur. No particular pattern of haemolysin production has been
associated with virulence.
a-Haemolysin (a-toxin) is a hydrophobic, surface-active protein with (apparently) no enzymic activity. It shows the Arrhenius effect: it is inactivated on heating to 60 C but is partly
reactivated on further heating to ca. 100 C. a-Haemolysin is
>100 times more effective against rabbit RBCs than human
RBCs. It appears to bind to the cell membrane, causing release
of K+ possibly due to the formation of transmembrane pores
by amphiphilic hexamers of the haemolysin. a-Haemolysin can
be lethal for man and animals; depending on animal species, it
can be leucocidal (= the NeisserWechsberg LEUCOCIDIN), can
aggregate and lyse blood platelets, and has a range of toxic
effects e.g. on the nervous and vascular systems (e.g. it increases
vascular permeability). When injected subcutaneously it can
have dermonecrotic effects which may be due to direct necrotizing activity or to prolonged vasospasm. a-Haemolysin has been
shown to play a major role in the pathogenesis of gangrenous
mastitis in sheep and cattle.
b-Haemolysin (b-toxin) is a SPHINGOMYELINASE C specific
for sphingomyelin (or lysolecithin); it is inactivated at 60 C,
requires Mg2+ for activity, and is inhibited e.g. by Zn2+
and chelating agents. It can hydrolyse the sphingomyelin in
sphingomyelin-rich RBCs (e.g. those from sheep or ox) without causing haemolysis; however, lysis can subsequently be
induced by chilling (see HOTCOLD LYSIS) or by the addition of
the CAMP factor (see CAMP TEST). b-Haemolysin is most frequently produced by staphylococci isolated from animals other
than man. Reports that it can be lethal are controversial. It is not
dermonecrotic (although it may cause necrosis in lactating mammary gland), but it can show toxic effects on the cardiovascular
Haemophilus
haemolytic system indicates the amount of complement (if any)
remaining unfixed in each dilution at the end of the first stage
in a CFT. (See also EAC.)
haemolytic uraemic syndrome (HUS) A potentially fatal disease
(of children and adults) involving renal impairment/acute renal
failure (see also TNF). An early stage of (bloody) diarrhoea
is common, though not invariably present. Most cases with
prodromal diarrhoea appear to be caused by O157 strains of
Escherichia coli (see EHEC) or by Shigella dysenteriae.
The major symptoms of HUS are toxin-dependent; attempts
are being made to sequester toxins in the gut (see SYNSORB Pk ).
Complications may include e.g. CNS involvement. Antibiotics
have not been found useful, and may be actually harmful.
Non-diarrhoeal HUS is sometimes associated with EHEC but
may be induced by certain drugs (e.g. mitomycin C, quinine),
and there are several other distinct causes.
haemophagocytic syndrome (HS) A syndrome which is characterized by fever and e.g. (commonly) cytopenia, coagulopathy,
hepatosplenomegaly and haemophagocytosis i.e. phagocytosis
of haemopoietic cells by HISTIOCYTES. Primary HS is associated
with inherited conditions. Secondary HS may be associated with
certain infections, malignancy or non-malignant conditions (e.g.
autoimmune disease), or may be drug-associated (phenytoin).
Infection-associated HS (IAHS) includes virus-associated HS
(VAHS) and bacterium-associated HS (BAHS).
The pathogenesis of HS is not understood but it appears to
involve unregulated T lymphocytes, monocytes, macrophages
and cytokines; elevated levels of e.g. IFN-g (interferon-g)
and IL-18 (interleukin-18) have been found in serum, and an
imbalance in Th1/Th2 cells has also been reported. Some 60%
of cases have been reported to occur in patients with preexisting immunodeficiency, suggesting that immune status may
be important as a predisposing factor.
Diagnosis includes demonstrating phagocytosis of erythrocytes (red blood cells), leukocytes and platelets by examination
of bone marrow.
Microorganisms associated with HS include: EpsteinBarr
virus (apparently responsible for most cases of VAHS) and other
herpesviruses (e.g. cytomegalovirus, HHV6 and HHV8); species
of Borrelia, Brucella, Mycobacterium, Rickettsia, Staphylococcus and Streptococcus; Cryptococcus; and Leishmania donovani.
[Haemophagocytic syndrome associated with infections: BCH
(2000) 13 163178.]
Haemophilus A genus of Gram-negative bacteria of the PASTEURELLACEAE. Cells: pleomorphic coccobacilli, rods (often ca.
0.4 12 m) or especially under suboptimal growth conditions filaments. Some strains have capsules. Fimbriae occur
in haemagglutinating strains (H. parasuis, H. paragallinarum,
strains of H. aegyptius). Optimum growth temperature: 3537 C.
Growth may require the X FACTOR and/or the V FACTOR (see PORPHYRIN TEST and SATELLITE PHENOMENON). Media for primary isolation include e.g. CHOCOLATE AGAR, FILDES ENRICHMENT AGAR, or
LEVINTHALS MEDIUM; some species (e.g. H. ducreyi, H. parasuis)
require serum. Growth in some species (e.g. H. aphrophilus,
H. paragallinarum) requires, or is enhanced by, incubation with
510% CO2 . Colonies on rich media are usually non-pigmented
or slightly yellowish, 0.52.0 mm diameter (48 hours/37 C);
those of capsulated strains are more mucoid and may appear
iridescent in obliquely transmitted light. Most species produce
acetic, lactic and succinic acids (usually without gas) from glucose. Most strains do not ferment lactose. NO3 is reduced to
NO2 ; NO2 may also be reduced. GC%: 3744. Type species:
H. influenzae.
Indole
Urease
ODCa
+
+
+
+
+
+
+
+
+
DECARBOXYLASE TESTS).
capsules, and six serotypes are distinguished on the basis of capsular antigens (polysaccharides, at least some of which contain
ribosyl groups). Strains of serotype b (usually biotype I) may
cause acute diseases such as CELLULITIS, EPIGLOTITIS, MENINGITIS
(in children), and PNEUMONIA (caused also by other serotypes).
Antisera to serotype b cross-react with antigens from a wide
range of bacteria e.g. staphylococci, streptococci, Bacillus spp.
Non-capsulated strains (usually biotypes II or III) occur as commensals (e.g. in the nasopharynx) but can occasionally cause
chronic conditions such as BRONCHITIS, CONJUNCTIVITIS, OTITIS
MEDIA and SINUSITIS. [Conjugate vaccine against H. influenzae
type b (for protection against e.g. meningitis and epiglottitis);
RMM (1996) 7 231241.]
H. paragallinarum (including strains formerly called H. gallinarum). Causes coryza in fowl. Requires V factor but not X
factor. Indole ve; urease ve; non-haemolytic; acid (no gas)
from glucose and (some strains) xylose; catalase ve.
H. parainfluenzae. Commensal in man, occasionally implicated in e.g. endocarditis. Requires V factor but not X factor.
Indole ve; urease ve (biotype I) or +ve (biotypes II and III);
non-haemolytic; acid (gas; biotype III: no gas) from glucose
but not from xylose; catalase +ve/ve.
H. parasuis (including most strains formerly called H. suis or
H. influenzae-suis). Causes GLASSERS DISEASE in pigs. Requires
353
haemoproteins
V factor but not X factor. Indole ve; urease ve; nonhaemolytic; acid (no gas) from glucose but not from xylose;
catalase +ve.
H. piscium. A fish pathogen (see ULCER DISEASE) now regarded
as an atypical strain of Aeromonas salmonicida.
H. vaginalis: see GARDNERELLA.
Other species: H. aphrophilus, H. avium, H. haemoglobinophilus, H. haemolyticus, H. paracuniculus, H. parahaemolyticus,
H. paraphrohaemolyticus, H. paraphrophilus, H. pleuropneumoniae, H. segnis. Species incertae sedis: H. somnus,
H. agni and H. equigenitalis, pathogenic in cattle, sheep and
horses, respectively.
[Book ref. 22, pp. 558569.]
haemoproteins See HAEM.
Haemoproteus A genus of protozoa of the HAEMOSPORORINA.
Species are parasitic in e.g. birds; the vectors are hippoboscid
flies.
haemorrhagic colitis COLITIS associated with bloody diarrhoea;
when caused by EHEC it usually occurs without fever.
haemorrhagic enteritis of turkeys An acute disease of turkeys
(particularly turkey poults 612 weeks of age) caused by an
AVIADENOVIRUS. Symptoms: depression, loss of appetite, bloody
faeces; haemorrhages also occur in the muscles and internal
organs. The disease may be fatal. [Book ref. 116, pp. 537539.]
(cf. MARBLE SPLEEN DISEASE.)
haemorrhagic fever with renal syndrome See HANTAVIRUS.
haemorrhagic fevers See VIRAL HAEMORRHAGIC FEVERS.
haemorrhagic nephrosonephritis Syn. KOREAN HAEMORRHAGIC
FEVER.
haemorrhagic septicaemia (1) (in fish) See INFECTIOUS DROPSY
and EGTVED DISEASE. (2) (barbone) An acute, often fatal, septicaemic CATTLE DISEASE which appears to be a primary PASTEURELLOSIS caused by strains of Pasteurella multocida. Onset
is sudden, with fever, profuse salivation, and petechial haemorrhages in submucosal tissues; death may occur within ca. 1 day.
A carrier state occurs. A vaccine is available.
haemorrhagic syndrome See TRICHOTHECENES.
Haemosporina See HAEMOSPORORINA.
Haemospororina A suborder of protozoa (order EUCOCCIDIORIDA) previously classified as the suborder Haemosporina (sic) of
the order Eucoccida [JP (1964) 11 720] or Eucoccidiida [JP
(1980) 27 3758]. In this suborder the organisms lack a conoid,
syzygy does not occur, and motile zygotes are formed (cf. ADELEORINA, EIMERIORINA); some species form pigment from host cell
haemoglobin (cf. PIROPLASMASINA). The organisms are heteroxenous, the asexual phase taking place in a vertebrate host and the
sexual phase occurring in a blood-sucking insect. Genera: e.g.
HAEMOPROTEUS, LEUCOCYTOZOON, PLASMODIUM.
haemotropic (haematotropic; hemotropic; hematotropic) Having
an affinity for the blood. (Used e.g. of blood parasites such as
Plasmodium.)
haemozoin (malarial pigment) A brown or black pigment which
occurs in the intraerythrocytic schizont of Plasmodium spp
(see PLASMODIUM and MALARIA). Haemozoin derives from the
erythrocytes haemoglobin; the parasite ingests haemoglobin,
uses the protein part, and (normally) detoxifies the remaining
ferriprotoporphyrin IX (FP) by polymerizing it to haemozoin.
(Unless detoxified by polymerization, FP can lyse the parasites
membranes.)
Haemozoin remains behind in the parasitized erythrocyte
following release of merozoites.
354
Halomonas
some species lyse (owing to weakening of the cell envelope
rather than to an osmotic effect per se).
The organisms are chemoorganotrophs which use amino acids
and/or carbohydrates as principal sources of carbon, and which
typically grow aerobically; metabolism is respiratory (oxidative).
The organisms form menaquinones rather than ubiquinones.
Under microaerobic or anaerobic conditions some strains can
use light energy (see PURPLE MEMBRANE; see also PHOTOTAXIS).
Two genera: HALOBACTERIUM (the type genus) and HALOCOCCUS.
Halobacterium A genus of catalase-positive, oxidase-positive
archaeans of the HALOBACTERIACEAE. The cells are lophotrichously flagellated (or non-motile) frequently pleomorphic rods
or filaments, or discs; they often contain gas vacuoles (which are
plasmid-encoded in at least some strains), and they lyse in dilute
solutions (e.g. NaCl ca. 0.81.5 M). Binary fission occurs by
constriction.
Most strains can be cultured in e.g. well-aerated tryptone yeast extract salt media. Optimum growth temperature:
4050 C.
Some strains form a PURPLE MEMBRANE under microaerobic or
anaerobic conditions.
The DNA in Halobacterium spp is often composed of a major
component (ca. 6090% of the total DNA) with a GC% of
ca. 6668, and a minor component (satellite DNA or plasmid
DNA) with a GC% of ca. 5760. Type species: H. salinarium.
H. halobium. See H. salinarium.
H. pharaonis. Motile, alkalophilic (optimum pH: 8.5) rods
which do not use sugars; substrates include e.g. formate,
fumarate, pyruvate. Growth occurs optimally in 3.5 M NaCl.
H. saccharovorum. Motile rods which form acid (mainly
acetic acid) from sugars. Growth occurs optimally in 3.54.5 M
NaCl.
H. salinarium (= H. halobium). Motile, typically rod-shaped
cells which grow aerobically or (strains with a purple membrane)
anaerobically in the light. Amino acids are used for carbon and
energy, although growth may be stimulated by carbohydrates
(without acid formation). Growth occurs optimally in 45 M
NaCl.
H. vallismortis. Motile, very pleomorphic rods which use
sugars, often with the formation of acid. Facultatively anaerobic.
Growth occurs optimally in 4.3 M NaCl.
H. volcanii. Mainly discoid or cup-shaped cells which are
(apparently) non-flagellated but which are sometimes capable
of a rotatory movement. Sugars are used for carbon and energy.
Growth occurs optimally in 1.52.5 M NaCl.
halocarbon See FREON.
halocins See BACTERIOCINS.
Halococcus A genus of catalase-positive and oxidase-positive
archaeans of the HALOBACTERIACEAE. The cells are non-motile,
orange- or red-pigmented cocci (diameter ca. 0.81.5 m) which
occur in pairs or in regular or irregular groups. At least
2.5 M NaCl is needed for growth; growth occurs optimally in
3.54.5 M NaCl. The organisms are much more resistant than
are Halobacterium spp to hypotonic solutions. Amino acids
are used for carbon and energy. Optimum growth temperature:
3037 C. GC%: ca. 6166. Type species: H. morrhuae [Book
ref. 22, pp. 266267].
halofantrine See MALARIA.
halogens (as antimicrobial compounds) See entries CHLORINE,
FLUORIDES, IODINE.
Halomonas A genus (incertae sedis) of aerobic, facultatively
anaerobic, chemoorganotrophic, halotolerant, Gram-negative
functions of the agropine strains are carried not by the Ri plasmid but by another plasmid which can cointegrate with it [MGG
(1983) 190 204214].
[Book ref. 55, pp. 271286.]
hairy shaker disease Syn. BORDER DISEASE.
halazone See CHLORINE.
half-a-Gram stain A non-specific staining procedure used e.g.
for detecting cells of Legionella in smears of sputum or aspirates
etc. The slide is flooded for 0.51 min with a solution of crystal
violet, drained, and flooded with Grams iodine solution for
12 min. The slide is then rinsed well in tap-water and dried
in air. (cf. GRAM STAIN.)
half-chiasma See RECOMBINATION.
half-reduction potential See REDOX POTENTIAL.
Halicystis See DERBESIA.
Halidrys See PHAEOPHYTA.
Halimeda
A genus of siphonaceous, mainly tropical or subtropical green seaweeds (division CHLOROPHYTA). The thallus
is segmented and calcified, and contains both chloroplasts and
amyloplasts. The cell wall contains a xylan (see XYLANS) as the
main structural component, and is more or less heavily calcified
with aragonite. When mature, the entire thallus is converted to
gametangia, after which it dies. Related holocarpic, usually calcified algae include species of CAULERPA, PENICILLUS and UDOTEA.
Haliscomenobacter
A genus of Gram-negative, rod-shaped
bacteria which occur e.g. in activated sludge. Individual cells
are apparently non-motile; they commonly occur in sheathed
trichomes. The organisms can utilize a range of carbon and
nitrogen sources; PHB is not formed. H. hydrossis has a GC%
of ca. 49. [Book ref. 45, pp. 425440 (436439).]
hallucinogenic mushrooms Certain agarics whose fruiting bodies contain hallucinogenic compounds; they include certain
species of Conocybe, Psilocybe (e.g. P. mexicana, P. semilanceata) and Stropharia. At least some of these fungi contain
psilocybin and/or psilocin, hallucinogenic tryptamine derivatives
related to serotonin. Some species of Lycoperdon also contain
hallucinogenic substance(s).
halo blight A typically seed-borne disease of beans (Phaseolus)
caused by Pseudomonas phaseolicola. Small, translucent lesions
on leaves later darken, each becoming surrounded by a yellowish
halo; leaves later exhibit interveinal yellowing, and brownish
spots may develop on pods.
halo spot A CEREAL DISEASE, caused by Selenophoma donacis
(Septoria oxyspora) which can affect e.g. barley, wheat and
rye. Small, pale lesions, each with a purplish-brown margin,
occur mainly on the leaves, and rows of dark-coloured pycnidia
develop in line with the veins. (Halo spot is called eyespot in
some parts of the world: cf. EYESPOT sense 2.)
halobacteria (1) Strains or species of Halobacterium. (2) Members of the family Halobacteriaceae.
Halobacteriaceae A family of extremely halophilic archaeans
which occur e.g. in salt lakes, evaporated brines, and salted
fish (in which they can cause spoilage). Cells: rods, cocci or
discs, containing orange, red or mauve carotenoid pigments
(predominantly bacterioruberins). Division occurs by binary
fission. The Gram reaction is negative. (See also CELL WALL,
GAS VACUOLE and S LAYER.)
Growth requires a minimum concentration of 1.5 M NaCl,
good growth typically needing 34 M NaCl; cells accumulate
electrolyte (mainly KCl) to an intracellular concentration at least
equivalent to that in the environment. High concentrations of
electrolyte are required to maintain the structural integrity of e.g.
the cytoplasmic membrane and the ribosomes; in dilute solutions
355
halonitrosoureas
bacteria which occur e.g. in salterns and (presumably) in salt
lakes etc. Cells: non-pigmented or yellow-pigmented, polarly
or laterally flagellated rods, 0.60.8 1.61.9 m, sometimes
pleomorphic or filamentous. Metabolism may be respiratory
(oxidative), with O2 or nitrate (anaerobic respiration) as terminal electron acceptor, or fermentative; anaerobic growth, without
nitrate, can occur with glucose but not with other carbohydrates.
Carbon sources include a wide range of alcohols, amino acids,
organic acids and sugars. Salt (NaCl) tolerance: 0.132.5%
w/v. Catalase +ve. Oxidase +ve. GC%: ca. 60. Type species:
H. elongata. [Book ref. 22, pp. 340343.]
halonitrosoureas See N-NITROSO COMPOUNDS.
halo-opsin See OPSIN.
halophile An organism which grows optimally only in the presence of electrolyte (commonly NaCl) at concentrations above
ca. 0.2 M, and which typically grows poorly, or not at all, in low
concentrations of electrolyte; examples include e.g. species of
ACTINOPOLYSPORA, DACTYLOCOCCOPSIS, HALOBACTERIUM, HALOCOCCUS, PARACOCCUS and VIBRIO. (cf. HALOTOLERANT.)
A number of authors have accepted the following categories: slightly halophilic (optimum growth in the presence of
0.20.5 M electrolyte); moderately halophilic (optimum growth
in 0.52.5 M electrolyte); extremely halophilic (optimum growth
in >2.5 M electrolyte).
[Halophilic and halotolerant organisms: Book ref. 157, pp.
171214, and Book ref. 191, pp. 5581.]
Halopteris See PHAEOPHYTA.
halorhodopsin A RETINAL-containing protein pigment (MWt ca.
25000) which occurs in the PURPLE MEMBRANE of Halobacterium
salinarium and which is involved in transmembrane ion translocation. Maximum absorption appears to occur at ca. 580 nm,
the absorption characteristics being stabilized by anions (primarily Cl ). On illumination, halorhodopsin undergoes cyclical
changes in its absorption characteristics with a periodicity of ca.
510 msec; several photointermediates appear to be involved.
Halorhodopsin undergoes bleaching when illuminated in the
presence of hydroxylamine. Some strains of Halobacterium salinarium (e.g. JW-5, W-296), which cannot synthesize retinal,
produce bacterio-opsin but are repressed in the synthesis of haloopsin.
Halothrix See PHAEOPHYTA.
halotolerant Refers to the ability of a non-HALOPHILE to grow
in the presence of high concentrations of electrolyte (e.g. up
to ca. 2.5 M); examples of halotolerant organisms include e.g.
HALOMONAS and strains of Staphylococcus.
Halteria A genus of freshwater ciliates (order OLIGOTRICHIDA).
Cells: roughly spherical, with very conspicuous oral ciliature
and a number of groups of cirri or bristles forming an
equatorial band. H. grandinella is ca. 2550 m in diam., has
a bouncing type of movement, and occurs e.g. in ponds and
organically polluted waters (see SAPROBITY SYSTEM) where it
feeds on bacteria; the organism is fairly tolerant of low O2 levels,
but is sensitive to NH3 and H2 S.
ham See CURING (1); MEAT SPOILAGE; SOFT CORE HAM.
hamanatto (black beans) An oriental food made by fermenting
whole soybeans with strains of Aspergillus oryzae. Beans are
steamed, coated with wheat flour, inoculated with A. oryzae, and
incubated 12 days. Brine and spices are added and incubation
is continued 612 months; the beans are then dried.
hamathecium A term which refers, collectively, to the various
types of structure which may occur between and around the asci
in an ascocarp: see e.g. PARAPHYSIS, PARAPHYSOID, PSEUDOPARAPHYSIS and PERIPHYSES.
HBB
(persistently infected) rodents including rats (Seoul virus),
mice (Sin Nombre virus, Dobrava-Belgrade virus, Hantaan virus)
and voles (Puumala virus); human infection appears to occur
mainly by inhalation of aerosols of the infected urine, faeces
etc. of rodents.
Species of Hantavirus include: Hantaan virus (HFRS; see also
KOREAN HAEMORRHAGIC FEVER), Seoul virus (HFRS), Puumala
virus (HFRS), Dobrava-Belgrade virus (HFRS), Sin Nombre
virus (HPS), Andes virus (HPS), Black Creek Canal Virus (HPS)
and Laguna Negra virus (HPS).
[Hantaviruses (persistence in rodent reservoirs): TIM (2000)
8 6167. Hantaviruses (review): JMM (2000) 49 587599.]
Haploangium See MYXOBACTERALES.
haploid Having a PLOIDY of one. (cf. DIPLOID, POLYPLOID.)
haploidization (mycol.) See PARASEXUAL PROCESSES.
haplokinety (1) The infraciliary base (only) of a stichodyad
PARORAL MEMBRANE. (2) A stichodyad paroral membrane.
haplomycosis Syn. ADIASPIROMYCOSIS.
haplont (1) (noun) An organism in whose life cycle only the
zygote is diploid. (cf. DIPLONT.) (2) The haploid form of an
organism, e.g. a gametophyte (see ALTERNATION OF GENERATIONS).
(3) (haplontic) (adj.) Refers to either (1) or (2) above.
haplophase In organisms which reproduce sexually: the haploid
phase of the life cycle. In many higher fungi haplophase and
DIPLOPHASE are separated by DIKARYOPHASE.
Haplospora See PHAEOPHYTA.
Haplosporangium See ADIASPIROMYCOSIS.
Haplosporidium A genus of protozoa (class STELLATOSPOREA)
which are parasitic in various aquatic invertebrates (including
annelids and molluscs). The spores are operculate and characteristically bear filamentous extensions which arise from the outer
spore coat and are typically coiled around the spore. [Spore ultrastructure in H. lusitanicum: J. Parasitol. (1984) 70 358371.]
The vegetative stage is plasmodial.
haplosporosomes See STELLATOSPOREA.
hapten A substance which can elicit an immune response only
when combined with another molecule or particle (carrier );
if administered on its own it fails e.g. to stimulate antibody
production (but cf. autocoupling hapten, below). The free
hapten can, however, combine with antibodies raised against
the haptencarrier complex; such combination may or may not
result in the precipitation of the haptenantibody complex. A
substance which acts as a hapten in one species may act as
a complete antigen in another e.g. the pneumococcal capsular
polysaccharides are haptenic in the rabbit but antigenic in man. A
hapten may be artificially bound to a protein in order to increase
the immunological specificity of that protein. Autocoupling
haptens bind spontaneously to tissue carriers in vivo, thus
becoming antigenic. (See also ALLERGEN.)
hapteron See CYATHUS.
haptocyst An EXTRUSOME in the tentacles of suctorian ciliates.
haptonema A thread-like appendage present on unicellular algae
of the PRYMNESIOPHYCEAE. Structurally, a haptonema bears some
resemblance to a eukaryotic FLAGELLUM but contains fewer
microtubules (which are arranged differently from those in a
flagellum) and has a sheath composed of several concentric
membranes, the innermost enclosing the microtubules. Haptonemata range from relatively short (e.g. in Prymnesium parvum)
to very long (>80 m in Chrysochromulina spp); most haptonemata (but not that of Prymnesium) can coil and uncoil:
e.g., in Chrysochromulina spp the haptonema remains coiled
while the organism is swimming and becomes extended when
the cell comes to rest. The haptonema is believed to function as
an attachment organelle.
HBcAg
GroES, GroEL and DnaK seem to prevent misfolding or aggregation of unfolded proteins, while the Lon protease degrades
abnormal proteins.
The heat-shock genes constitute a REGULON composed of
several unlinked operons (for example: promoterdnaK dnaJ
and promotergroES groEL). The heat-shock regulon is under
the control of a positive transcriptional activator encoded by
gene rpoH (previously called htpR). RpoH (MWt ca. 32000)
is a SIGMA FACTOR (s32 ) which interacts with RNA POLYMERASE,
producing a holoenzyme (Es32 ) that promotes transcription
from heat-shock promoters more efficiently than does Es70 .
(Transcription of the rpoH gene itself requires Es70 [JB (1986)
166 380384].)
Following heat shock, the increased levels of RpoH are
due mainly to increased translation of the protein rather to
increased transcription of rpoH. The heat-induced translation
from rpoH mRNA involves an effect of temperature on a
secondary structure formed in the mRNA by base-pairing
between a site immediately downstream of the start codon (a
downstream box ) and another region in the coding sequence.
This secondary structure normally inhibits translation, but on
temperature upshift it is destabilized so that translation can
occur; thus, the mRNA acts as a thermosensor (an RNA
thermometer ) for expression of s32 [GD (1999) 13 633636].
Although synthesized under normal conditions, s32 has a short
half-life (about 1 min); it appears that, within the cell, s32 forms
complexes with DnaK, DnaJ and GrpE and is subsequently
degraded by the FtsH protease. During heat shock DnaK binds
preferentially to denatured proteins leaving RpoH free to
function as a sigma factor [EMBO (1996) 15 607617].
The heat-shock response in other bacteria. In some bacteria
the mechanism for regulating the heat-shock response differs
from that in E. coli. In some cases there is a regulatory sequence
upstream of heat-shock genes; this inverted repeat sequence,
termed CIRCE (controlling inverted repeat of chaperone expression), occurs e.g. in strains of Bacillus and Clostridium and is
also found in some Gram-negative bacteria. In Bradyrhizobium
japonicum the control mechanism includes at least two distinct
regulatory systems involving CIRCE and a s32 -like sigma factor
[JB (1996) 178 53375346].
More recently it has been reported that control of the heatshock response involves negative regulation by repressor proteins (in conjunction with cis-acting DNA sequences) which
inhibit transcription of the HSP genes under normal physiological conditions [Mol. Microbiol. (1999) 31 18].
(See also SOS SYSTEM.)
Strains of E. coli mutant in the rpoH gene have been useful
in the OVERPRODUCTION of recombinant proteins.
heated lid cycler See THERMOCYCLER.
heavy chain A class-specific polypeptide IMMUNOGLOBULIN component (MWt ca. 5000070000, depending on Ig class). The
various types of heavy chain are designated alpha, gamma, delta,
epsilon and mu corresponding to Ig classes IgA, IgG, IgD, IgE
and IgM, respectively. In IgM, different C-terminal sequences
occur in the heavy chains of the membrane-associated and pentameric forms. Certain Ig classes can be divided into subclasses
on the basis of minor differences in their heavy chains.
heavy metals (and their compounds) (as antimicrobial agents)
Although trace amounts of certain heavy metal ions are essential for the growth of microorganisms, higher concentrations may
exhibit antimicrobial activity. Heavy metal ions bind to certain
groups (particularly thiol groups) and appear to exert antimicrobial activity largely by inactivating proteins, nucleic acids and
RNA synthesis. HBB-resistant mutants emerge rapidly; HBBdependent mutants have also been isolated.
HBcAg See HEPATITIS B VIRUS and HEPATITIS B.
HBeAg See HEPATITIS B VIRUS and HEPATITIS B.
HBsAg See HEPATITIS B VIRUS and HEPATITIS B.
HBV HEPATITIS B VIRUS.
HCAM Syn. CD44.
HCC HEPATOCELLULAR CARCINOMA.
HCMV Human cytomegalovirus: see BETAHERPESVIRINAE.
HCV HEPATITIS C VIRUS.
HCVs (human caliciviruses) See SMALL ROUND STRUCTURED VIRUSES.
HD protein Helix-destabilizing protein (see SINGLE-STRAND BINDING PROTEIN).
HD50 (CH50 ; C H50 ) Haemolytic dose (50%): the quantity of
COMPLEMENT needed to lyse 50% of a standardized suspension
of sensitized erythrocytes. In a COMPLEMENT-FIXATION TEST the
HD50 may be used as the unit in place of MHD (q.v.); this gives a
more accurate end-point (since the graph %lysis of cells versus
quantity of complement is sigmoidal).
HDAg See DELTA VIRUS.
HDCV Human diploid cell vaccine (see RABIES).
hDNA Hybrid DNA. (See e.g. CLONING.)
H-DNA See TRIPLEX DNA.
HE-cellulose (HEC) Hydroxyethylcellulose: a neutral cellulose
derivative sometimes used in preference to CM-CELLULOSE in
CELLULASE assays.
HE markers See TRANSFORMATION (1).
headful mechanism A mechanism of genome packaging during
virion assembly: packaging is initiated by insertion into a
prohead (or provirion) of one end of a concatemeric form of the
genome (which, at or before insertion, may be cut at a particular
sequence); incorporation of the genome then continues until the
head is full. Thus, termination of packaging is determined only
by the length of the nucleic acid packaged, and not by a specific
sequence in the nucleic acid. (See e.g. BACTERIOPHAGE MU and
BACTERIOPHAGE P22; cf. e.g. BACTERIOPHAGE l.)
Heaf test A form of TUBERCULIN TEST. PPD is spread over a
small area of skin and is then pressed into the skin with a Heaf
gun: an instrument which punctures the skin with several small
needles.
heart rot See TREE DISEASES.
heartwater See COWDRIA.
heat-fixed smear See FIXATION.
heat-shock proteins (HSPs) Proteins which are synthesized at
greatly (but transiently) increased levels in an organism in
response to a sudden rise in temperature or to certain other types
of stress (e.g. ultraviolet radiation, virus infection, ethanol, or the
intracellular accumulation of abnormal proteins); HSPs may be
necessary for survival of the organism at higher temperatures,
and they are produced at the expense of normal proteins. Such
a heat-shock response has been observed in a wide range of
species from bacteria and yeasts to plants and animals; at least
some HSPs have been highly conserved through evolution, but
the response is regulated differently in different organisms.
In Escherichia coli there are at least 17 HSPs which include
the products of genes dnaJ, dnaK, groEL, groES, rpoD, lysU and
lon. Synthesis of these proteins reaches a peak ca. 510 min
after a rise in temperature (for example, 30 42 C), and subsequently declines to a new steady state which is greater than
that at the lower temperature. Some HSPs apparently cope with
stress-induced damage for example, the molecular chaperones
358
Helicobacter
Helicases I and III both act processively and move in the 5 -to3 direction along the strand to which they are bound. Helicase
I is encoded by the traI gene of the F plasmid [PNAS (1983)
80 46594663]; it seems to be responsible for nicking at oriT
in the F plasmid [JBC (1991) 266 1623216237], and may
be involved in unwinding the plasmid DNA for transfer during
CONJUGATION (sense 1b). Helicase III cannot replace either the
Rep protein or helicase II.
Some bacteriophages encode their own helicases; for example,
the dda gene product of phage T4 is a helicase, while the gp4 of
phage T7 is a protein with both helicase and PRIMASE activities.
The DnaB helicase, which is active e.g. in DNA replication,
is a ring-shaped hexamer of DnaB proteins [see e.g. Cell (1996)
86 177180].
Helicobacter A genus of asporogenous Gram-negative bacteria
classified within the e (epsilon) subdivision (= rRNA superfamily
VI) of the taxon Proteobacteria (which also includes the family
CAMPYLOBACTERACEAE). The cells are typically curved/helical
rods with one or more sheathed flagella (unsheathed e.g. in
H. pullorum). Currently there are 20 named species, many of
which have been isolated from the intestines (and often liver)
of animals (e.g. dogs, sheep, pigs, rodents, chickens). However,
attention has been focused primarily on the species H. pylori
owing to its association with e.g. gastritis and peptic-ulcer disease
in humans.
H. pylori was formerly classified within the genus Campylobacter, but was re-classified [IJSB (1989) 39 397405]. Cells:
curved/helical, ca. 0.50.9 m wide and up to 3 m in length;
motile (several flagella). Genome: circular, approx. 1700 kb;
GC%: average 39, but significant differences occur in specific regions one such region including the cag PATHOGENICITY ISLAND [H. pylori strain 26695 (complete genome): Nature
(1997) 388 539547].
Chemoorganoheterotrophic. Microaerophilic. Culture on enriched media (e.g. blood, chocolate agar) needs high humidity
(freshly poured, undried plates) and a gaseous phase of e.g.
oxygen/carbon dioxide/nitrogen (5%/10%/85%); grey, translucent colonies (<2 mm in diam.) are obtained after 37 days
at 3537 C. The medium may be made selective for H. pylori
by adding e.g. amphotericin, nalidixic acid and vancomycin (to
which the organism is resistant).
Oxidase +ve, catalase +ve, urease +ve.
The pathogenesis of H. pylori -associated gastric disease is
not understood. One suggestion was based on the presence of
lipopolysaccharide antigens identical to the Lewis x and Lewis
y antigens found e.g. in human gastric mucosa; it was postulated
that these antigens might provoke an antibody response and
give rise to autoimmune inflammation [molecular mimicry of
H. pylori : TIM (1997) 5 7073]. However, this idea was
questioned because the predominant anti-LPS antibodies found
in a number of infected patients were unrelated to the given LPS
antigens [Inf. Immun. (1998) 66 30063011].
Pathogenesis seems likely to involve the cag pathogenicity
island and an unlinked gene, vacA, which is often jointly
expressed. The joint expression of cag and vacA (in type I
clinical strains) appears to correlate with severe gastrointestinal
disease, while type II strains (which lack cag, and do not express
vacA) are generally not associated with severe disease.
The reason why infection with H. pylori gives rise to gastric
cancer in only some individuals may depend on host genetic
factors such as polymorphisms which affect levels of the proinflammatory cytokine interleukin-1b (IL-1b) [Nature (2000)
404 398402].
Helicobasidium
the period between successive initiations of DNA replication; it
is equal to the doubling time. As each I period ends, another I
period begins.
The principle of the HelmstetterCooper model is illustrated
in the figure. Some of the factors that may influence or determine
the length of the I period are indicated in the entry CELL CYCLE.
Helotiales An order of fungi (subdivision ASCOMYCOTINA) which
are typically saprotrophs or plant parasites. Ascocarp: APOTHECIOID with paraphyses, sessile or stipitate, sometimes setose.
Asci: unitunicate, typically cylindrical; inoperculate, but with
an apical pore. Ascospores: typically not elongated. Genera:
e.g. Ascocoryne, Botryotinia, Bulgaria, Chlorociboria (see also
GREEN OAK), Chlorosplenium, Ciboria, Dasyscyphus, DIPLOCARPON, Geoglossum, Korfia, Microglossum, Mitrula (see also
MYCOPARASITE), Monilinia, Pezizella (see also MYCORRHIZA),
Phacidium (see also SNOW BLIGHT), SCLEROTINIA, Spathularia,
Trichoglossum.
helotism (mycol.) Literally: serfdom. The term has been used to
refer to the (supposedly) subservient role of the photobiont in a
LICHEN.
helper component (plant virol.) See NON-CIRCULATIVE TRANSMISSION.
helper T cell See T LYMPHOCYTE.
helper virus Any virus which can provide functions necessary
for the replication of a DEFECTIVE VIRUS or e.g. of a SATELLITE
RNA.
Helvella A genus of fungi (order PEZIZALES) in which the ascocarp is a stipitate APOTHECIUM which is typically saddle-shaped
(saddle fungi); the smooth to warty, guttulate ascospores are
commonly colourless or pale brown.
helveticin J See BACTERIOCINS.
heme See HAEM.
Hemiascomycetes A class of ascomycetes characterized by the
formation of naked asci (i.e., asci not formed on or in an
organized ascocarp) which do not develop from a system of
ascogenous hyphae; the hemiascomycetes include most of the
yeasts (e.g. Saccharomyces spp) and e.g. Taphrina spp. The class
is not recognized in most modern taxonomic schemes; most of
the hemiascomycetes are now placed in the ENDOMYCETALES.
Hemiaulus See DIATOMS.
Hemibasidiomycetes See TELIOMYCETES.
hemicelluloses The non-cellulosic polysaccharide fraction
obtained from isolated plant cell walls by extraction with alkali
after the PECTIC POLYSACCHARIDES have been extracted. Hemicelluloses are closely (but non-covalently) associated with CELLULOSE and occur in the matrix of the plant cell wall; they include
e.g. galactomannans, glucomannans (see MANNANS), mixed bglucans, XYLANS, xyloglucans etc.
hemidesmosome See TRYPANOSOMA.
Hemidiscus A genus of DIATOMS which are generally regarded
as centric, although the valves are often markedly asymmetric.
Blooms of H. hardmannianus in estuarine and neritic waters
in India have been associated with high mortalities of fish and
invertebrates [Limn. Ocean. (1985) 30 910911].
Hemileia See UREDINIOMYCETES and COFFEE RUST.
hemimethylated DNA dsDNA in which only one of the strands
is methylated (see DNA METHYLATION).
Hemitrichia A genus of slime moulds (class MYXOMYCETES).
H. serpula forms conspicuous, yellowish, sessile, reticulate
plasmodiocarps (up to several centimetres across) on humus or
on rotting wood.
Hemming filter An apparatus used for FILTRATION. Two bijou
bottles are clamped together, mouth-to-mouth, with a filter
(a)
Slow growth
Rapid growth
(b)
D
I
D
I
I
HELMSTETTERCOOPER MODEL (see entry). (a) Chromosome replication during growth at different rates (cells and chromosomes are
represented diagrammatically). Replication begins at a specific location in the chromosome, the origin, which is shown here as a small circle.
During slow growth (upper sequence) each new daughter cell has exactly one chromosome because, following duplication of the parental
chromosome, a new round of replication does not begin before the parent cell has divided fully.
During faster growth (lower sequence), a new round of replication has begun before the previous round has been completed well before
cell division; as a result, each new daughter cell has fractionally more than one chromosome.
(b) The cell division cycle may be represented as a linear sequence of three periods: I, C and D. C is the period during which chromosome
replication occurs. D is the period in which the septum forms cell division occurring at the end of the D period. I is the period between each
successive initiation of chromosomal replication. Each I period starts when the previous one ends. (Continued on page 362.)
361
hemp retting
it consists of a circular (but not covalently closed), partially
double-stranded DNA molecule in which one strand (the L,
long, or () strand) is of fixed length (ca. 30003300
nucleotides long) and has unique 3 and 5 ends and a protein
(the DNA-linked protein) covalently attached to the 5 end. The
other strand (the S, short, or (+) strand) has a fixed 5 end but
a variable 3 end, and varies in length from 50 to 100% of that of
the L() strand. (The 3 end of the S(+) strand can be extended
by the endogenous viral polymerase, the L() strand acting as
template.) The circularity of the molecule is maintained by basepairing between the 5 ends of the two strands (the cohesive
overlap); in all hepadnaviruses there is an 11-bp direct repeat
sequence on either side of the cohesive overlap.
In mammalian hepadnaviruses, the L() strand has four open
reading frames, orientated in the same direction, designated S,
C, P and X regions. The S region comprises the S gene, the preS1 region and the pre-S2 region; it encodes the major protein
(S gene), middle protein (pre-S2 + S gene) and large protein
(pre-S1 + pre-S2 + S gene) of the viral envelope. The C region
comprises the C gene (which encodes the major core protein) and
the pre-C region. The product of the P region (which overlaps
the whole of the S region and parts of the C and X regions)
is a large histidine-rich protein (MWt ca. 90000) which is a
DNA polymerase with REVERSE TRANSCRIPTASE activity. The X
region includes the cohesive overlap sequence and encodes a
polypeptide of unknown function. (DHBV lacks an X region.)
The viral genes are expressed via at least two unspliced primary
transcripts. No known viral protein is encoded by the S(+)
strand.
Hepadnavirus DNA replication occurs by a characteristic
mechanism involving reverse transcription of an RNA intermediate (see RETROID VIRUSES). When a virion infects a host cell, the
viral DNA enters the nucleus and is converted to a supercoiled
ccc dsDNA molecule. The L() strand is transcribed to form
multiple copies of a 3.5-kb RNA called the pre-genome; this
RNA is then encapsidated with the viral DNA polymerase and
DNA-linked protein, and an L() strand of DNA is synthesized
by reverse transcription of the pre-genome. The pre-genome
is then apparently degraded by an RNase H activity, and an
S(+) strand is synthesized on the L() strand template. The
DNA-linked protein may act as primer for L() strand DNA
synthesis, while a small fragment of RNA may be the primer
for S(+) strand synthesis. (cf. RETROVIRIDAE.) The assembly of
the virions and their release from the cell can occur before
S(+) strand synthesis is complete, accounting for the partially
double-stranded nature of the genome in virions liberated into
the bloodstream.
[Review (mainly of HBV): Nature (1985) 317 489495; Book
ref. 110, pp. 2341.]
heparin A highly sulphated proteoglycan present e.g. in MAST
CELLS and other cells. Heparin varies in MWt according e.g.
between them; one bijou contains the sample, the other acts
as the receiving vessel. On centrifugation, liquid passes through
the filter into the receiver.
hemp retting See RETTING.
Henneguya
A large genus of protozoa (class MYXOSPOREA)
which are important histozoic parasites in various fish. Species
are commonly specific for a given host and for a particular
tissue within that host: e.g. the Channel catfish (Ictalurus punctatus) may be parasitized by H. adiposa (adipose fin), H. diversis
(liver and kidney), or H. exilis (gills), while the Pacific salmon
(Oncorhynchus spp) can be infected by H. salminicola (muscles). Typically, conspicuous spore-filled cysts (up to 15 mm
across in e.g. salmon infected with H. salminicola) are formed.
Heavy infestations may kill the fish (particularly when the gills
are affected).
HEP High egg passage: refers to the number of times that a given
strain of virus has undergone SERIAL PASSAGE in eggs. (See e.g.
FLURY VIRUS; cf. LEP.)
HEp-2 (H.Ep2, Hep-2, hep-2 etc) An ESTABLISHED CELL LINE
derived from a human laryngeal carcinoma; the cells are heteroploid and epithelioid. HEp-2 cultures support the replication
of a wide range of viruses.
HEPA filter High-efficiency particulate air filter, used e.g. in a
SAFETY CABINET.
Hepadnaviridae A family of enveloped DNA-containing animal viruses which can cause hepatitis in man, animals or
birds; the family includes HEPATITIS B VIRUS (HBV) of man,
GROUND SQUIRREL HEPATITIS VIRUS (GSHV), DUCK HEPATITIS B
VIRUS (DHBV), and WOODCHUCK HEPATITIS VIRUS (WHV) [Intervirol. (1986) 25 1429], and probably tree squirrel (Sciurus
carolinensis pennsylvanicus) hepatitis B virus (THBV) [PNAS
(1986) 83 29942997]. These viruses closely resemble one
another in structure and genetic organization, but differ e.g. in
their interactions with their hosts. The hosts immune response
to hepadnavirus infection has been implicated in the pathology
of the virus-induced liver disease. Although all of the hepadnaviruses are highly hepatotropic, HBV DNA has also been
detected in e.g. pancreatic, spleen and kidney cells, and DHBV
can apparently infect duck pancreatic and kidney cells.
The infectious hepadnavirus virion (ca. 42 nm diam.) consists
of a nucleocapsid (an internal core containing the viral genome)
surrounded by a lipoprotein envelope. The core contains a major
protein (designated P22C in HBV) and is associated with a DNA
polymerase and a protein kinase which can phosphorylate the
major core protein. In HBV, at least, the envelope contains three
proteins: a major protein (glycosylated form: GP27S , nonglycosylated form: P24S ), the middle protein (two glycosylated
forms: GP33S and GP36S ), and the large protein (glycosylated
form: GP42S ; non-glycosylated form: P39S ).
The genome, as present in hepadnavirus virions isolated from
the blood of an infected host, has a characteristic structure:
362
hepatitis B virus
Lab. diagnosis involves detection of HBV antigens in the
serum. HBsAg (see HEPATITIS B VIRUS) appears in the serum during the incubation period and persists through the symptomatic
phase of the disease. It usually begins to disappear ca. 23
months after the onset of symptoms; if it persists for >6 months,
the patient has become a carrier and may develop chronic liver
disease. Anti-HBsAg antibodies appear only late in convalescence; the high levels of HBsAg present in the blood may induce
immune tolerance to this antigen. HBeAg appears in the serum
just before symptoms begin; its appearance is associated with
high infectivity and the presence of whole (infectious) virions
(Dane particles) in the blood. HBcAg does not appear in the
serum, but anti-HBcAg antibodies can be detected as symptoms
begin. Anti-HBcAg IgM antibodies disappear late in the convalescence phase, but anti-HBcAg IgG antibodies may persist
for years (possibly for life), and detection of the latter is a useful indicator of previous infection. [Screening blood samples for
HBV by PCR: Lancet (1999) 353 359363.]
Treatment. There is no specific treatment for the clinical disease. Antiserum may be used for pre- or post-exposure prophylaxis. Vaccines containing HBsAg are available [PM (1984)
75 199211].
hepatitis B virus (HBV) A virus of the HEPADNAVIRIDAE (q.v.)
which causes HEPATITIS B in man, and which is also apparently a
causal agent of human hepatocellular carcinoma (HCC). (HBV
can also infect chimpanzees, but does not cause chronic hepatitis
or HCC in these animals.) (cf. WOODCHUCK HEPATITIS VIRUS.)
On infection of a new host (see HEPATITIS B), the HBV virion
attaches to the surface of a hepatocyte and penetrates the cell
by endocytosis or by fusion of the viral envelope with the
host cell plasma membrane. HBV surface (envelope) antigen
(HBsAg) and core antigen (HBcAg) become associated with the
plasma membrane of the infected cell, and subsequently large
amounts of HBsAg are released into the circulation in the form
of non-infectious (DNA-free), spherical or tubular lipoprotein
particles (ca. 22 nm diam.). HBsAg (formerly known e.g. as
Australia antigen, Au antigen, or hepatitis-associated antigen,
HAA) is a dimer of two molecules, linked by disulphide bonds,
of the envelope major protein (see HEPADNAVIRIDAE). HBcAg
is the major capsid polypeptide (P22C ). The soluble e antigen
(HBeAg) is a product of proteolytic cleavage of HBcAg. The
appearance in the serum of infected individuals of antibodies to
these antigens provides a useful means of monitoring disease
development (see HEPATITIS B).
HBV strains can be serotyped on the basis of their HBsAg.
HBsAg contains a group-specific determinant (designated a),
common to all subtypes, together with subtype-specific determinants (designated d, y, w and r ); strains typically contain either
d or y with either w or r. The four principal serotypes, which
differ in geographical distribution, are adw, adr, ayw and ayr.
The subtype determinants are useful epidemiological markers.
In ca. 510% of individuals infected with HBV, HBsAg persists in the circulation for >6 months, and a carrier state is
established which may persist for life. The carrier state may
be asymptomatic (latent infection) or symptomatic (with e.g.
chronic active hepatitis, cirrhosis, and/or HCC), and is most
likely to develop in e.g. perinatally-infected or immunodeficient
individuals. In HBV carriers, viral DNA may integrate at one
or more (apparently random) sites in the host cell genome; the
integrated sequences may be complete genomes or subgenomic
fragments, and in HCC cells they are often extensively rearranged, with e.g. multiple deletions, inversions, duplications, etc.
Rearrangements also occur in the flanking cellular sequences.
to the methods used for its isolation; that used as an ANTICO(heparin inhibits thrombin activity) has a MWt of
ca. 25000. In addition to anticoagulant activity, heparin can
e.g. modify (limit) delayed hypersensitivity reactions in mice
and guinea pigs (mechanism unknown), stimulate phagocytosis, inhibit the alternative pathway of complement fixation (by
enhancing the activity of Factor H), and inhibit eosinophilmediated ADCC. Heparin is cleaved by heparinases, and its
activity can be neutralized by e.g. protamines.
hepatitis Inflammation of the liver. Hepatitis is often caused by
viruses (e.g. HEPATITIS A, HEPATITIS B, HEPATITIS C); hepatitis D and
hepatitis E viruses are less-common causal agents. The significance of infection with hepatitis G virus is currently uncertain
[transfusion-associated hepatitis G virus infection: NEJM (1997)
336 747754; RMM (1998) 9 207215]. Hepatitis may also
occur as a symptom of non-viral infectious diseases (see e.g.
amoebic DYSENTERY). [Diagnostic perspective of viral hepatitis:
RMM (1997) 8 197207.]
hepatitis A (infectious hepatitis; epidemic hepatitis; short-incubation hepatitis) A viral HEPATITIS caused by the hepatitis A
virus (HAV, = ENTEROVIRUS type 72); it tends to occur in
epidemics among children and young adults, particularly in
closed institutions (e.g. mental hospitals). Man is probably the
only natural host, but certain other primates (e.g. chimpanzees)
can be infected. A carrier state is not known. Infection occurs
mainly by consumption of water, milk or food contaminated with
human faeces e.g. shellfish harvested from sewage-polluted
waters. HAV replicates in hepatocytes and is presumed to
reach the intestine (and hence faeces) via the bile duct. The
peak excretion of virus occurs during the latter half of the
incubation period (26 weeks). Symptoms: fatigue, anorexia,
low-grade fever, some abdominal pain, and sometimes jaundice.
The disease is usually self-limiting within a few weeks; rarely, a
severe, fulminant, often fatal hepatitis develops. Lab. diagnosis:
demonstration of HAV in faeces; serological tests for anti-HAV
IgM antibodies in serum.
hepatitis B (serum hepatitis; homologous serum jaundice; longincubation hepatitis) A viral HEPATITIS caused by the HEPATITIS
B VIRUS (HBV). Incubation period: 26 months (but occasionally
as short as 2 weeks). Infection occurs by direct inoculation or by
contamination of mucous membranes. The virus is present in the
blood and body fluids (saliva, semen, mucus, wound exudates
etc) of an infected person. Transmission may thus occur by the
transfusion of blood or blood products from infected donors;
by tattooing, ear-piercing, vaccination, renal dialysis, etc, using
contaminated needles; by sexual contact; or (in infants) during
birth. (Intrauterine infection is uncommon since HBV does not
normally cross the placenta.) HBV reaches the liver via the blood
and replicates in the hepatocytes. The disease may be mild or
subclinical, and a carrier state is recognized (see HEPATITIS B
VIRUS). In clinical cases, onset is gradual with jaundice and e.g.
nausea, malaise, pains in muscles and joints, with or without
fever; occasionally acute hepatic failure occurs. (See also DELTA
VIRUS.) Pathogenesis appears to involve the hosts immune
response to viral antigens in the plasma membranes of infected
hepatocytes. The condition may be self-limiting, or chronic liver
disease may develop; chronic infection is associated with an
increased risk of hepatocellular carcinoma (HCC: see HEPATITIS
B VIRUS) and possibly other tumours, including KAPOSIS SARCOMA
[JAMA (1984) 251 10071008]. HCC is a major cause of death
in regions where HBV is endemic and neonatal infection is
common (e.g. in regions of China and tropical Africa).
AGULANT
363
hepatitis C
Six major genotypes and >60 subtypes of HCV have been
distinguished. Treatment of hepatitis C is apparently influenced
by the specific genotype involved and the level of viraemia;
disease caused by genotype 2 or 3, in conjunction with low-level
viraemia, is reportedly more likely to respond in a sustained
fashion to treatment with IFN-a, while disease caused by
genotype 1 or 4 is apparently more refractory.
[Quantification of HCV in plasma samples: JCM (1997) 35
187192.]
In many cases HCV causes persistent infection. Persistence
may be facilitated by the relatively poor immunogenicity of the
virus and the low-level viraemia. Changes in viral antigens, due
e.g. to mutations in HVR-1, may also contribute to persistence;
however, genetic drift in HCV may be independent of the hosts
(weak) immune pressure [JV (2000) 74 25412549].
(See also CD81.)
hepatitis D, E See HEPATITIS.
hepatitis D virus Syn. DELTA VIRUS.
hepatitis delta virus Syn. DELTA VIRUS.
hepatitis G virus See HEPATITIS.
hepatitis X Hepatitis in dogs caused by ingestion of food
contaminated with AFLATOXINS; the liver becomes necrotic and
congested, with haemorrhagic oedema of the gall bladder
mucosa.
hepatocellular carcinoma (HCC) A CARCINOMA of liver cells.
Primary HCC can be caused e.g. by HEPATITIS B VIRUS and
WOODCHUCK HEPATITIS VIRUS. (See also HEPATITIS C.)
hepatotoxin A TOXIN which acts on the liver.
hepatotropism See TROPISM (sense 2).
HEPES A zwitterionic pH buffer: N-2-hydroxyethylpiperazineN -2-ethanesulphonic acid. HEPES is widely used e.g. in TISSUE
CULTURES, and has also been used in bacterial cultures; it is
readily soluble in water, and does not bind divalent cations such
as Ca2+ , Mg2+ or Cu2+ . At 37 C the pKa of HEPES is ca. 7.3;
at 25 C it is ca. 7.5. (cf. BICINE.)
Herberts pits See TRACHOMA.
herbicolin A An acyl peptide antibiotic produced by Erwinia
herbicola. It can inhibit the growth of yeasts and filamentous
fungi, and can kill sterol-requiring mollicutes [JAC (1985) 16
449455]; it is inactive against other bacteria.
herbivorous Refers to protozoa which feed on bacteria and/or
algae. (cf. CARNIVOROUS.)
herd immunity See EPIDEMIOLOGY.
herd structure See EPIDEMIOLOGY.
Heribaudiella See PHAEOPHYTA.
Hericium A genus of fungi of the APHYLLOPHORALES.
hermaphroditism The phenomenon in which an individual has
both male and female sexual organs; such an individual may
exhibit HOMOTHALLISM or HETEROTHALLISM.
herpangina An acute (usually self-limiting) infectious PHARYNGITIS, occurring mainly in children and young adults, caused by
coxsackieviruses A2A6, A8 and A10. Small, vesicular, ulcerating lesions develop in the pharyngeal region, and there may
be varying degrees of fever and/or prostration.
herpes (1) Any disease caused by a herpesvirus (especially
HERPES SIMPLEX but also e.g. HERPES ZOSTER) and characterized
by the formation of small vesicular lesions on skin and mucous
membranes. (2) Used increasingly as a synonym of genital
herpes (see HERPES SIMPLEX).
herpes genitalis See HERPES SIMPLEX.
herpes gladiatorum See HERPES SIMPLEX.
herpes labialis See HERPES SIMPLEX.
herpes simplex An infectious disease, caused by herpes simplex
virus (HSV) type 1 or 2 (see ALPHAHERPESVIRINAE), which
herpes zoster
chickenpox, such lesions may appear before development of the
characteristic skin lesions.) [Virology of the mouth (including
HSV infections): RMM (1994) 5 209216.]
Lab. diagnosis. For infections other than encephalitis: scrapings from the edges of lesions, or biopsies from skin or liver,
are examined microscopically for multinucleate giant cells with
eosinophilic intranuclear inclusion bodies; HSV can be demonstrated e.g. by immunofluorescence techniques, ELISA etc.
For encephalitis, laboratory diagnosis may be made e.g.
by PCR-based examination of cerebrospinal fluid (CSF), thus
avoiding the risks of brain biopsy [see e.g. JCM (1997) 35
691696]. The PCR-based detection of HSV (types 1 and 2)
may be facilitated by a commercial system involving the use of
MOLECULAR BEACON PROBES that hybridize to amplicons of both
HSV type 1 and HSV type 2 (HSVision ; Stratagene). (HSV
type 2 is not a common cause of viral encephalitis; it may be a
causal agent e.g. in immunocompromised individuals.)
Chemotherapy. A number of antiviral agents (e.g. ACYCLOVIR,
IDOXURIDINE, PENCICLOVIR, trifluorothymidine, VIDARABINE) are
active against HSV and are useful in some cases; for example,
vidarabine has been used in cases of HSV encephalitis, while
acyclovir, or penciclovir, is used in creams for the topical
treatment of lesions on skin and mucous membranes. In general,
such agents are not effective in preventing recurrence or
transmission.
herpes simplex virus group See ALPHAHERPESVIRINAE.
herpes zoster A human disease resulting from the reactivation
of a latent human (alpha) herpesvirus 3, present in a dorsal
nerve ganglion, subsequent to an attack of CHICKENPOX that
may have occurred (many) years earlier. The virus replicates in
the ganglion, and in adjacent nervous tissue, and is transported,
within the axon, to nerve endings in the corresponding region
of skin; viral replication is believed to account for pain experienced during the acute phase of the disease the pain being
accompanied by an eruption of characteristic clusters of vesicular lesions. (Lesions may develop in areas not served by the
affected nerves; this is thought to be due to viral dissemination
in the bloodstream.) (See also RAMSAY HUNT SYNDROME.) Reactivation of the virus may occur spontaneously or may be provoked
e.g. by immunosuppression, certain drugs, or other diseases.
Post-herpetic neuralgia (PHN) is prolonged pain which
appears to be due to damage sustained by the peripheral nervous system as a result of viral replication. Some regard PHN
as pain which persists following the disappearance of the rash,
while others have defined PHN as e.g. pain which persists for at
least 30 days from the onset of the rash. In an attempt to provide
a usable definition (for clinical trials of antiviral agents), the concept of zoster-associated pain (ZAP) has been introduced; ZAP
includes the continuum of acute and chronic pain.
Chemotherapy. The use of antiviral agents in the acute phase
of herpes zoster is generally beneficial, and is particularly important in immunocompromised patients in whom herpes zoster
may become a life-threatening condition; in the latter patients,
intravenous ACYCLOVIR is the first-choice therapy (which may
decrease the risk of dissemination).
For immunocompetent patients with moderate to severe pain
during the acute phase, systemic antiviral therapy should reduce
the duration of the rash and pain if given immediately after the
onset of the rash (within a maximum of 72 hours after onset);
useful drugs: ACYCLOVIR, FAMCICLOVIR, VALACICLOVIR (each of
which can be administered orally). Acyclovir should be given
intravenously if severe complication (e.g. encephalitis) develop.
[Treatment of zoster: RMM (1995) 6 165174.]
Herpesviridae
variety of criteria such as the disease caused by the virus (e.g.
Mareks disease virus, herpes simplex virus); CPEs induced by
the virus (e.g. cytomegalovirus); host species (e.g. Herpesvirus
saimiri ); names of pioneer workers (e.g. EpsteinBarr virus,
Lucke virus).
It has been recommended [Book ref. 139, pp 123] that the
name of a herpesvirus should usually be based on the family
or subfamily to which its primary host belongs (subfamily for
bovine and primate viruses, family in other cases) viruses
isolated from humans being prefixed by human; the name
may, where applicable, indicate the subfamily of herpesviruses
to which the virus belongs (alpha, beta or gamma), and is
followed by a number numbers being allocated sequentially
as new viruses are discovered. Thus, e.g. Mareks disease
virus becomes gallid herpesvirus 1; herpes simplex type 1
virus becomes human (alpha) herpesvirus 1; EpsteinBarr virus
becomes human (gamma) herpesvirus 4.
Many herpesviruses, including some important pathogens of
animals, were not listed in an earlier (1982) classification scheme
[Book ref. 23, pp 4751]. These viruses include e.g. bovine
herpesvirus 1 (causal agent of various cattle diseases, such
as INFECTIOUS BOVINE RHINOTRACHEITIS, encephalitis in newborn
calves, infectious pustular vulvovaginitis and abortion in cows
etc.); anatid herpesvirus 1 (= anserid herpesvirus1, causal agent
of DUCK VIRUS ENTERITIS); gallid herpesvirus 3 (causal agent of
AVIAN INFECTIOUS LARYNGOTRACHEITIS); herpesviruses of amphibians (e.g. Lucke virus, causal agent of renal adenocarcinoma in
frogs, Rana pipiens) [review: Book ref. 140, pp 367384]; and
herpesviruses of reptiles and fish (see e.g. CARP POX and CHANNEL
CATFISH VIRUS DISEASE) [review: Book ref. 140, pp 319366].
Herpesvirus ateles See GAMMAHERPESVIRINAE.
herpesvirus B Syn. B VIRUS.
Herpesvirus saimiri See GAMMAHERPESVIRINAE.
Herpesvirus simiae Syn. B VIRUS.
herpetic Pertaining to or caused by a herpesvirus see e.g.
HERPES SIMPLEX.
herpetic cervicitis See HERPES SIMPLEX.
herpetic stomatitis See HERPES SIMPLEX.
Herpetomonas A genus of homoxenous parasitic protozoa (family TRYPANOSOMATIDAE) which occur (typically in the gut) in flies,
bugs and hymenopterous insects. Promastigote, paramastigote
and opisthomastigote forms occur during the life cycle; biflagellate organisms may result from rapid division of promastigotes.
Herpetosiphon
A genus of GLIDING BACTERIA (see CYTOPHAGALES) which occur in aquatic (freshwater to marine) habitats.
The organisms are gliding filaments (up to ca. 2 m wide) which
may be sheathed; they typically contain carotenoid glycoside
pigments ranging from yellow or orange. Metabolism appears
to be chemoorganotrophic. GC%: ca. 4453.
Herpetosoma A subgenus of TRYPANOSOMA within the STERCORARIA; species include parasites of rodents and man. The trypomastigote form typically has a subterminal kinetoplast, a pointed
posterior end, and a free flagellum.
T. (H.) lewisi, a parasite in rats, is transmitted cyclically and
contaminatively by fleas, e.g. Xenopsylla cheopis; it is cultivable
e.g. in NNN medium at 2527 C. In the vertebrate host, the
reproductive forms (epimastigotes) undergo multiple fission or
unequal binary fission, resulting eventually in the production of
non-dividing trypomastigotes.
T. (H.) rangeli is parasitic in man (and in e.g. cats, dogs
etc) in Central and South America, and is transmitted cyclically mainly by bugs of the genus Rhodnius. Although classified in the Stercoraria, this species is transmitted by bite: the
heterokont
helps to maintain the anaerobic state. [Protection of nitrogenase from oxygen in heterocystous cyanobacteria: MR (1992)
56 352362.]
In Anabaena strain PCC 7120, which forms heterocysts
in both terminal and intercalary locations, differentiation of
heterocysts depends on a functional hetR gene. In genetically
engineered cells of this strain, controlled expression of hetR can
induce differentiation of heterocysts even under conditions that
would normally repress their formation. However, in cells with a
mutant patA gene which form heterocysts almost exclusively
at terminal locations the expression of hetR did not induce
the formation of intercalary heterocysts; this was interpreted to
mean that, while raised levels of HetR are necessary to promote
the formation of heterocysts, PatA may play a role in regulating
the expression of hetR [PNAS (2001) 98 27292734].
During nitrogen fixation, the heterocysts and vegetative cells
are metabolically interdependent. The vegetative cells supply
heterocysts with e.g. fixed carbon, reduced sulphur, and glutamate; in the heterocyst, fixed nitrogen is transferred to glutamate by glutamine synthetase (see AMMONIA ASSIMILATION),
and the resulting glutamine is passed back to vegetative cells
to supply their nitrogen requirements. Communication between
a heterocyst and adjacent vegetative cell(s) occurs via fine
pores (microplasmodesmata) in their juxtaposed cytoplasmic
membranes; juxtaposition of these membranes occurs at the
vegetative-cell end of a channel (the pore channel ) which passes
through the thick heterocyst envelope. (Microplasmodesmata are
also found between vegetative cells.) [Heterocyst differentiation
and function: Book ref. 75, pp. 219242, 265280.]
heterocytotropic antibodies CYTOPHILIC ANTIBODIES (particularly
REAGINIC ANTIBODIES) which can attach to the cells of two or
more different host species. (cf. HOMOCYTOTROPIC ANTIBODIES.)
heteroduplex Any double-stranded nucleic acid in which some,
or many, of the bases in one strand are not complementary to
bases in the corresponding positions in the other strand; such
mismatching of base pairs is reflected in the thermal stability
of the duplex. (See also DNA HOMOLOGY and HOMODUPLEX.)
The term heteroduplex is also used for any duplex in which
each strand originates from a different parent duplex (see e.g.
RECOMBINATION), even though such strands may in some cases
be strictly complementary.
heteroecious Syn. HETEROXENOUS.
heterofermentation (1) Any fermentation in which there is more
than one major end-product. (2) Syn. HETEROLACTIC FERMENTATION.
heterogeneous nuclear RNA See HNRNA.
heterogenote See MEROZYGOTE.
heteroglycan See POLYSACCHARIDE.
heteroimmune phages See SUPERINFECTION IMMUNITY.
heteroimmunization The stimulation of an immune response to
antigens derived from another species. (cf. ISOIMMUNIZATION.)
heterokaryon (heterocaryon) (mycol.) A hyphal cell, mycelium,
organism, or spore which contains genetically different nuclei.
(cf. HOMOKARYON.)
heterokaryosis (mycol.) The condition in which genetically different nuclei exist in the same cell, mycelium or spore; it may
arise e.g. by the entry of a genetically different nucleus into
a HOMOKARYON (e.g. by hyphal fusion) or by mutation in a
binucleate or multinucleate homokaryotic cell or mycelium. Heterokaryosis is important e.g. in PARASEXUAL PROCESSES.
heterokont Refers to a pair of flagella (on a biflagellate cell) in
which one flagellum differs from the other in length and often
also in type: see e.g. XANTHOPHYCEAE. (cf. ISOKONT.)
Heterokontae
heteroresistance (1) The resistance (of an organism) to two or
more related antibiotics e.g. two or more b-lactam antibiotics.
(2) See MRSA.
heterothallism The phenomenon in which sexual reproduction
requires the involvement of two different thalli an individual
thallus being self-sterile even when (as is common) it is
hermaphroditic; gametes etc which can unite sexually are said
to be compatible. (cf. HOMOTHALLISM; see also COMPATIBILITY
sense 2.)
In morphological heterothallism (= dioecism) compatibility
is determined solely on a sexual basis: there are separate male
and female thalli, and sexual reproduction can occur between
any male thallus and any female thallus of the same species.
Dioecism is uncommon among fungi; it occurs e.g. in some
species of Achlya and of Laboulbenia.
In physiological heterothallism male and female organs generally occur on the same thallus, and in these cases compatibility
is determined not only on a sexual (malefemale) basis: sexual
union can occur between male and female gametes etc only if
each has appropriate mating type allele(s) (see MATING TYPE);
gametes etc which have the same mating type allele(s) cannot
unite sexually and are said to be incompatible. In e.g. many
zygomycetes, male and female organs are not distinguishable;
in such cases sexually compatible thalli are often designated
plus and minus.
In bipolar physiological heterothallism compatibility is determined at one mating type locus which may contain either of 2
alleles; if these alleles be designated A and a, then mating can
occur between one individual (mating type) which has the A
allele and another which has the a allele. Bipolar heterothallism
is also called one-locus two-allele heterothallism, unifactorial
heterothallism (since only one locus is involved), or DIMIXIS
(since two alleles are involved).
In tetrapolar physiological heterothallism compatibility is
determined at two mating type loci, each locus containing one
of two alleles. If these loci be designated A, B (with alleles a,
b, respectively), four mating types can be distinguished: AB, Ab,
aB and ab. Mating can occur only between individuals which
contain complementary alleles at both loci; thus, e.g. mating can
occur between AB and ab individuals, and between Ab and aB
individuals. Tetrapolar heterothallism is also called bifactorial
heterothallism.
In some cases of one- and two-locus heterothallism, a locus
may be occupied by any allele of an allelomorphic series; in such
cases there can be many mating types. (See also DIAPHOROMIXIS.)
Heterothallism provides a constraint on inbreeding, and consequently increases the potential for genetic reassortment within
a species.
Heterotrichida An order of free-living and parasitic ciliate protozoa (class POLYHYMENOPHOREA) in which the organisms are
typically large, often contractile (see MYONEME), and sometimes
pigmented, and in which somatic ciliature is commonly abundant
and oral ciliature is well developed. Genera include e.g. Balantidioides, BLEPHARISMA, Brachonella, Bursaria, Condylostoma,
Metopus, SPIROSTOMUM and STENTOR.
heterotrichous (1) Having different types of cilia or flagella.
(2) Of certain filamentous algae: having a vegetative thallus
consisting of both prostrate and erect systems of filaments (as
e.g. in CHAETOPHORA).
heterotroph An organism which uses organic compounds for
most or all of its carbon requirements. (cf. AUTOTROPH; ORGANOTROPH.) The term heterotroph is often used to refer specifically to CHEMOORGANOHETEROTROPHS although chemolithotrophs and phototrophs may also be heterotrophic.
high-dry objective
reactions of the EMBDENMEYERHOFPARNAS PATHWAY; similarly,
glyceraldehyde 3-phosphate may be converted to pyruvate via
the latter part of the EMP pathway. In organisms with a functional TCA CYCLE, pyruvate can be oxidized to yield energy via
the TCA cycle and a respiratory chain. In organisms which lack a
complete TCA cycle, pyruvate may be converted to acetyl-CoA
and thence to acetic acid (as in some acetic acid bacteria). Alternatively, under certain conditions, glyceraldehyde 3-phosphate
can be converted to glucose 6-phosphate (by reactions of GLUCONEOGENESIS) which can then re-enter the HMP pathway; in this
case, for every six molecules of glucose entering the pathway,
one molecule is effectively completely oxidized. If reducing
equivalents from NADPH can be transferred to NAD+ (see
TRANSHYDROGENASE) and thence to an electron acceptor via a
respiratory chain, the pathway can be used to generate energy
even in the absence of a TCA cycle. Other functions of the
HMP pathway include the metabolism of those pentoses which
can be converted to intermediates of the pathway. (See also RMP
PATHWAY.)
hexulose phosphate pathway Syn. RMP PATHWAY.
hexuronic acids URONIC ACIDS corresponding to hexoses.
hexylresorcinol See PHENOLS.
hfl genes (in E. coli ) See BACTERIOPHAGE l.
hflB gene See FTSH.
Hfr donor High frequency recombination donor: a conjugal
donor (see CONJUGATION sense 1b) created by the insertion of a
CONJUGATIVE PLASMID (sense 1) into a bacterial chromosome. The
chromosome of an Hfr donor can be mobilized by the plasmid so
that chromosomal genes can be transmitted to a recipient during
conjugation; thus, in a mixed population of recipients and Hfr
donors, recombination between recipient and (transferred) donor
DNA will occur at high frequency in the recipient population.
The (relatively few) conjugative plasmids which can give rise
to Hfr donors include the F PLASMID.
A conjugative plasmid which cannot normally integrate into
the bacterial chromosome may be able to do so if it first integrates e.g. with the genome of an A+ B strain of BACTERIOPHAGE MU, integration of the plasmidMu complex into the
chromosome then being mediated by Mu; a recipient mated with
such an Hfr donor must be lysogenic for a c+ strain of Mu to
avoid ZYGOTIC INDUCTION when the Mu prophage is transferred
to the recipient.
(See also PRIME PLASMID and INTERRUPTED MATING.)
HFRS Haemorrhagic fever with renal syndrome (see HANTAVIRUS).
HFT (of plasmids) See EPIDEMIC SPREAD.
HFT lysate See TRANSDUCTION.
HGV Hepatitis G virus (see HEPATITIS).
HHV1 Human (alpha) herpesvirus 1 (see ALPHAHERPESVIRINAE).
HHV2 Human (alpha) herpesvirus 2 (see ALPHAHERPESVIRINAE).
HHV3 Human (alpha) herpesvirus 3 (see ALPHAHERPESVIRINAE).
HHV4 Human (gamma) herpesvirus 4 (see GAMMAHERPESVIRINAE).
HHV5 Human (beta) herpesvirus 5 (see BETAHERPESVIRINAE).
HHV6 Human (beta) herpesvirus 6 (see BETAHERPESVIRINAE).
HHV7 Human (beta) herpesvirus 7 (see BETAHERPESVIRINAE).
HHV8 Human (gamma) herpesvirus 8 (see GAMMAHERPESVIRINAE).
HI test HAEMAGGLUTINATION-INHIBITION TEST.
HIB HAEMOLYTIC IMMUNE BODY.
Hibitane See CHLORHEXIDINE.
high-dry objective Any objective lens which has a numerical
aperture between 0.65 and 0.95, and which is not used as an
immersion lens.
high-fructose corn syrup A sweetening agent produced industrially from glucose by GLUCOSE ISOMERASE (see also IMMOBILIZATION).
high-mobility group proteins See NON-HISTONE PROTEINS.
high mutability gene Syn. MUTATOR GENE.
high-performance liquid chromatography See CHROMATOGRAPHY.
high-potential ironsulphur protein See HIPIP.
high-pressure liquid chromatography See CHROMATOGRAPHY.
high zone tolerance See IMMUNOLOGICAL TOLERANCE.
higher fungi Fungi of the subdivisions ASCOMYCOTINA, BASIDIOMYCOTINA and DEUTEROMYCOTINA. (cf. LOWER FUNGI.)
Highlands J virus See ALPHAVIRUS.
highly active antiretroviral therapy See HAART.
HIGM See RNA EDITING.
Hikojima variant See VIBRIO (V. cholerae).
hilar appendix A small protuberance on a basidiospore near its
region of attachment to the sterigma.
Hildenbrandia See RHODOPHYTA.
Hill reaction In PHOTOSYNTHESIS: light-dependent evolution of
oxygen by isolated CHLOROPLASTS in the absence of CO2 but
in the presence of e.g. ferric oxalate which acts as an electron
acceptor for PS-II.
hilum The mark, scar or small projection on a spore corresponding to the region at which it was formerly attached to the
spore-bearing structure.
him genes (in E. coli ) See BACTERIOPHAGE l.
Himanthalia See PHAEOPHYTA.
Himmelweit pipette A PASTEUR PIPETTE with a hole in the side
of the capillary end; it is used e.g. in the harvesting of allantoic
fluid from an EMBRYONATED EGG.
hin gene See PHASE VARIATION.
HindII A RESTRICTION ENDONUCLEASE from Haemophilus influenzae; GTPy/PuAC.
HindIII A RESTRICTION ENDONUCLEASE from Haemophilus influenzae; A/AGCTT.
HinfI See RESTRICTION ENDONUCLEASE (table).
hinge region In the heavy chain of an IMMUNOGLOBULIN: the
amino acid sequence at the junction of the Fd portion and the
Fc portion; it appears to confer conformational flexibility on the
molecule. Structurally, the hinge region is the most variable part
of the constant region of the heavy chain. In alpha and gamma
chains (but not in mu chains) the hinge region is rich in proline.
Hinozan (edifenphos; O-ethyl-S,S-diphenyl phosphorodithioate)
An antifungal ORGANOPHOSPHORUS COMPOUND used as a protectant against rice blast disease; it can act e.g. as a powerful
cutinase inhibitor (see CUTIN).
hip gene (in E. coli ) See BACTERIOPHAGE l.
HiPIP High-potential ironsulphur protein: a type of IRONSULPHUR PROTEIN which has a single [4Fe4S] centre and a highly
positive Em ; the HiPIP in Chromatium vinosum has an Em of
+350 mV.
hippurate hydrolysis Certain bacteria (e.g. Streptococcus spp,
Campylobacter spp) produce a hippuricase which hydrolyses
hippurate (C6 H5 .CO.NH.CH2 .CO2 ) to benzoate and glycine.
Hippuricase activity may be detected by adding a calculated
amount of acid FeCl3 to a 4-day culture of the organism in a
medium containing 1.0% sodium hippurate; the FeCl3 forms a
persistent precipitate with benzoate (positive test). (A precipitate
is also formed with hippurate, but this is more soluble with
excess FeCl3 ; the amount of FeCl3 used in the test is that
which just dissolves the hippurate precipitate initially formed
in an uninoculated control tube on dropwise addition of the
370
HIV
lung function or to secondary bacterial infection. Infrequently,
histoplasmosis becomes disseminated (usually in young children
or in the elderly, debilitated or immunocompromised); lesions
may occur in lymph nodes, liver, spleen, intestine, skin, heart,
kidneys, CNS etc. Disseminated histoplasmosis is often rapidly
fatal. Lab. diagnosis: serological tests (e.g. a CFT); microscopic
and cultural examination of clinical specimens. Chemotherapy:
e.g. amphotericin B, ketoconazole.
histotope A site on an MHC class I or II antigen recognized by
a T lymphocyte.
histozoic Living (parasitic) within tissues. (cf. COELOZOIC.)
Histriculus See HYPOTRICHIDA.
hit-and-run oncogenesis Oncogenesis which is initiated by a
particular agent (e.g. a virus) but, once initiated, can proceed
in the absence of the initiating agent.
HIV Human immunodeficiency virus, infection with which can
give rise to AIDS (q.v.). HIV is a retrovirus (family RETROVIRIDAE)
classified within the subfamily LENTIVIRINAE. HIV was previously referred to as AIDS-associated retrovirus (ARV), HTLVIII (cf. HTLV), immunodeficiency-associated virus (IDAV) and
lymphadenopathy-associated virus (LAV).
Evidence for the involvement of HIV in AIDS was obtained
in 1983 [Science (1983) 220 868871]. Subsequently a distinct,
but related, retrovirus was detected in AIDS patients in West
Africa [Nature (1987) 326 662669]. These two viruses are now
designated HIV-1 and HIV-2 respectively. HIV-1 and HIV-2 are
similar in both structure and genome.
The origin of HIV is unknown. One hypothesis supposes that
the major (M) strain of HIV arose through the use of an antipoliomyelitis vaccine that had been prepared by culturing polio
virus in non-human primate cells; it is proposed that a simian
strain of immunodeficiency virus (initially present in the culture
cells) contaminated the vaccine and (thus) entered the vaccinated
human population (located mainly in the Congo) in the late
1950s. Subsequent studies on viruses from the Congo area do
not support this hypothesis [Nature (2001) 410 10471048].
The HIV virion is 100 m in diameter. Its innermost region
consists of a cone-shaped core that includes (i) two copies of
the (positive-sense) ssRNA genome, (ii) the enzymes REVERSE
TRANSCRIPTASE, integrase and protease, (iii) some minor proteins,
and (iv) the major core protein. The core is surrounded by a
protein matrix, and the whole is enclosed within an envelope
(a lipid bilayer); the envelope is penetrated by a number of
spikes (gp41), each spike bearing a distal (outermost) trimeric
glycoprotein (gp120). [Fine structure of HIV: Virol. (1987) 156
171176.]
The genome (9.2 kb) includes sequences corresponding to
the gag, pol and env regions of other exogenous retroviruses
(see RETROVIRIDAE).
The gag region encodes structural proteins, including the
major core protein (p24) and the matrix protein (p17).
The pol region encodes regulatory proteins: REVERSE TRANSCRIPTASE, protease (involved in the maturation of virions),
RNASE H and integrase. (The enzymes reverse transcriptase and
protease are major targets for antiretroviral drugs.)
The env region encodes the envelope-associated proteins,
gp120 (required for initial binding of virus to target cell)
and gp41 (involved in fusion of the viral envelope with the
membrane of the target cell).
Other HIV genes include: tat and rev (whose products are
needed for viral replication); vif (viral infectivity factor); and
vpu (whose product promotes efficient budding of the (HIV-1)
virion during productive infection of a cell). (See also Rev in
GENE THERAPY.)
HIV-positive
The LTR also includes a regulatory region for polyadenylation
of transcripts.
Synthesis of viral mRNA, and of genomic RNA, is carried
out by the hosts RNA polymerase. Viral envelope proteins are
translocated to, and insert into, the cell membrane (with gp120
located at the outer surface). The assembled core acquires an
envelope by budding through the cell membrane.
Culture.
Culture may be useful e.g. for diagnosis of HIV infection in
neonates; in these young patients the presence of anti-HIV
antibody may simply reflect acquisition from an HIV-positive
mother.
Cultures of HIV characteristically exhibit CPE (cytopathic
effects), including the formation of giant multinucleated cells
and cell lysis. Culture can be carried out in CD4+ T cells; the
virus can also infect other types of cell such as monocytes and
promyelocytes [Virol. (1985) 147 441448]. HIV may give rise
to a persistent, non-cytopathic and productive (virion-producing)
infection of human CD4+ T cells in culture [Science (1985) 229
14001402].
Inactivation of HIV by disinfection.
Hypochlorite (effective conc. 10000 parts per million available
chlorine) is a useful disinfectant. Glutaraldehyde (dangerous
chemical!!!) has been used for disinfecting surfaces in a wellventilated environment; safety regulations must be observed.
Phenolics and ethanol are unsuitable.
In serum, inactivation of HIV may require more than
30 minutes at 56 C [e.g. Book ref. 219, p 814].
Genetic variability of HIV isolates.
Isolates of HIV from different patients tend to be genetically
heterogeneous, particularly in the env sequence [minireview:
Cell (1986) 46 14], and variation may also be observed in
isolates obtained sequentially from the same patient over a period
of time [Science (1986) 232 15481553]. As env encodes
the (antigenic) viral surface protein gp120, such ANTIGENIC
VARIATION presents a problem for the development of an effective
anti-HIV vaccine; in this context, studies have been carried out to
determine the effect of genetic variation on the immunogenetic
potential of gp120 [Arch. Virol. (2000) 145 20872103].
HIV-positive Refers to an individual who is infected with the
human immunodeficiency virus (see HIV). (See also AIDS.)
hives Syn. URTICARIA.
Hjarres disease (coli-granuloma) A POULTRY DISEASE in which
granulomatous lesions are formed in the wall of the intestine
(particularly in the caecum); the causal agent is Escherichia coli.
HLA-A, HLA-B etc. See MAJOR HISTOCOMPATIBILITY COMPLEX.
Hly plasmid See ESCHERICHIA.
HlyA (of Escherichia coli ) See RTX TOXINS.
HMA Hydroxymethionine analogue: DL-a-hydroxy-g-methiolbutyrate; HMA is used in animal feedstuffs as a sulphur amino acid
supplement [ARB (1983) 52 215216]. (See also SINGLE-CELL
PROTEIN.)
HMG box That region, in certain types of protein, which can
e.g. interact with sharply angular or kinked DNA (in eukaryotic
cells); it consists of a sequence of about 80 amino acid residues
(including a high proportion of aromatic amino acids) with a net
positive charge. HMG boxes are found in certain NON-HISTONE
PROTEINS. (See also HU PROTEIN.)
HMG proteins See NON-HISTONE PROTEINS.
HMP pathway HEXOSE MONOPHOSPHATE PATHWAY.
HMS-1 b-lactamase See b-LACTAMASES.
HMT toxin A long-chain polyketide host-specific toxin produced
by Drechslera (Helminthosporium) maydis race T; it has been
suggested that HMT toxin acts as an ionophore.
homogenote
hnRNA Heterogeneous nuclear RNA: the high-MWt RNA synthesized by RNA polymerase II in the nucleus of a eukaryotic
cell; hnRNA occurs in the form of ribonucleoprotein (hnRNP)
and includes pre-mRNA (i.e., MRNA before the generation of 3
ends, polyadenylation and splicing).
H-NS protein (syn. H1 protein) In bacteria (e.g. Escherichia
coli ), a small protein (136 amino acids, 15.6 kDa) encoded
by the hns gene. H-NS protein is able to (i) regulate the
expression of various unrelated genes (e.g. bgl, proU ), (ii)
constrain negative supercoiling, and (iii) contribute to the
physical organization of the bacterial nucleoid.
In uropathogenic strains of E. coli (UPEC) the H-NS protein
has been implicated in the temperature-dependent expression
of P FIMBRIAE: at the non-permissive temperature of 25 C,
the H-NS protein is reported to act as a methylation-blocking
factor, repressing transcription [Mol. Microbiol. (1998) 28
11211137]. In Proteus mirabilis it is reported to act as a
repressor of the transcriptional activator gene, ureR, in the
absence of urea induction [JB (2000) 182 26492653].
H-NS has also been implicated in the regulation of DNA repair
in Shigella [JB (1998) 180 52605262].
H-NS protein is able to condense supercoiled plasmid DNA,
and appears to play a major part in condensing DNA in
the nucleoid. H-NS-mediated condensation of DNA has been
investigated by studying the structure of H-NSDNA complexes
by atomic force microscopy [NAR (2000) 28 35043510].
Hoarella A genus of protozoa (suborder EIMERIORINA) which
form dizoic oocysts each containing 16 sporocysts.
Hoechst 33258 A bis-benzimidazole derivative: a FLUOROCHROME
used e.g. for staining chromosomes.
hog cholera Syn. SWINE FEVER.
hog diseases See PIG DISEASES.
Hogness box See PROMOTER.
holdfast An organ or organelle by means of which an organism or
cell attaches to the substratum or to another organism. Examples
include the root-like region of LAMINARIA, and the specialized
regions in SPORICHTHYA and members of the ASTOMATIDA.
holdingflush jar procedure In the culture of anaerobes: a
procedure which minimizes the exposure of plates to O2 ;
essentially, uninoculated plates, or inoculated plates awaiting
incubation, are held in an anaerobic jar (with unclamped lid)
while a stream of O2 -free gas (e.g. N2 or CO2 ) is continually
directed through a tube to the bottom of the jar.
holin See LYSIS PROTEIN.
Hollandina See SPIROCHAETALES.
Holliday junction See RECOMBINATION.
Holliday model See RECOMBINATION (Figure 1).
Holliday structure See RECOMBINATION.
Holmsella A genus of algae (division RHODOPHYTA). H. pachyderma is a colourless organism which is parasitic on the red
alga Gracilaria; PIT CONNECTIONS have been observed between
H. pachyderma and Gracilaria.
Holobasidiomycetidae A subclass of fungi (class HYMENOMYCETES) characterized by the formation of holobasidia (see
BASIDIUM). Orders [Book ref. 64, p. 189]: AGARICALES, APHYLLOPHORALES, BOLETALES, BRACHYBASIDIALES, CANTHARELLALES,
DACRYMYCETALES, EXOBASIDIALES, RUSSULALES and TULASNELLALES.
holobasidium See BASIDIUM.
holoblastic development See CONIDIUM.
holocarpic Refers to those organisms in which the entire thallus
takes on a reproductive function. (cf. EUCARPIC.)
holocellulose A complex of cellulose and hemicelluloses (formed
e.g by the removal of lignin from lignocellulosic plant material).
homoglycan
homoglycan See POLYSACCHARIDE.
homoheteromixis See HOMOTHALLISM.
homoimmune phages See SUPERINFECTION IMMUNITY.
homoiomerous (homoeomerous) (1) (lichenol.) Refers to a lichen
thallus in which the photobiont is more or less evenly distributed
throughout the thallus (see LICHEN). (2) (mycol.) In an agaric:
refers to a pileus or stipe composed of hyphae only. (3) (ciliate
protozool.) See MACRONUCLEUS. (cf. HETEROMEROUS.)
homoisocitrate pathway See icl SERINE PATHWAY.
homokaryon (homocaryon) (mycol.) A hyphal cell, mycelium,
organism or spore in which all the nuclei are genetically
identical. (cf. HETEROKARYON.)
homokaryotic (1) (mycol.) Refers to a HOMOKARYON. (2) (ciliate
protozool.) Having only one type of nucleus: see PRIMOCILIATID
GYMNOSTOMES.
homolactic fermentation A type of LACTIC ACID FERMENTATION
in which e.g. glucose is converted entirely, or almost entirely,
to lactic acid. Many LACTIC ACID BACTERIA (e.g. Lactococcus
lactis, thermobacteria and streptobacteria) carry out a homolactic fermentation of glucose (or lactose) under conditions of
glucose (or lactose) excess (cf. LACTIC ACID STARTERS); glucose
is metabolized by the EMBDENMEYERHOFPARNAS PATHWAY, and
most or all of the pyruvate thus formed is converted to lactic acid. (See also LACTOSE.) However, under glucose or lactose
limitation, or with different substrates (e.g. PENTOSES), the same
organisms may form other products, sometimes with little or no
lactic acid; for example, many strains of L. lactis produce mainly
formic and acetic acids and ethanol when grown in glucose- or
lactose-limited continuous culture (see Appendix III(c)). (See
also DIACETYL.)
homologous (1) Similar in form or structure, but not necessarily in function; homology suggests evolutionary relatedness.
(2) Derived from or associated with the same species as that
being referred to. (cf. HETEROLOGOUS (1).) (3) See ALTERNATION
OF GENERATIONS. (4) (immunol.) The antibody elicited by a given
antigen is said to be homologous to that antigen; similarly, the
antigen is said to be homologous to the antibody. (cf. HETEROLOGOUS (3).) (5) (genetics) Of chromosomes or chromatids:
containing the same sequence of genes but not necessarily
identical alleles. (6) (genetics) Of nucleic acids: see e.g. DNA
HOMOLOGY.
homologous interference See INTERFERENCE (1).
homologous recombination See RECOMBINATION.
homologue (of chromosomes) In a diploid eukaryotic nucleus:
each of a pair of CHROMOSOMES which encode the same types of
characteristics and which are usually morphologically similar;
in general, homologous chromosomes carry the same sequences
of genes, though not necessarily the same alleles.
homology (of DNA) See DNA HOMOLOGY.
homomixis See HOMOTHALLISM.
homonym Any name used to refer to each of two (or more)
different microbial taxa; a name of a higher animal or plant
which is identical to that of a microorganism is not considered to
be a homonym. The name published first is the senior homonym,
while any name published later is a junior homonym; junior
homonyms are usually suppressed.
homophilic binding (of cell adhesion molecules) See IMMUNOGLOBULIN SUPERFAMILY.
homoplasmid segregant See INCOMPATIBILITY.
homopolymer tailing See TAILING.
homopolysaccharide See POLYSACCHARIDE.
homoserine See e.g. Appendix IV(d).
homothallism (homomixis) Self-fertility: the phenomenon in
which sexual reproduction can involve the fusion of e.g. gametes
hotcold lysis
rigid particles (ca. 100150 20 nm) composed of ssRNA and
helically-arranged subunits of a single type of coat protein (MWt
ca. 21000). The genome appears to consist of 24 molecules
(depending on strain) of linear positive-sense ssRNA, two or
three of which are necessary for infection. The 3 end of the
RNA has an internal poly(A) sequence and a 3 -terminal tRNAlike structure which can be amino-acylated with tyrosine in vitro
[Virol. (1982) 119 5158]. Viruses accumulate mainly in the
cytoplasm but also in the nuclei of infected cells. Type member:
barley stripe mosaic virus (BSMV), an important pathogen of
barley in many regions of the world; some strains of BSMV
can also infect wheat, oats etc. Transmission is mechanical
and seed-borne. Seeds from BSMV-infected plants may show
increased frequencies of triploidy and aneuploidy, and some
BSMV strains induce a heritable genetic anomaly (aberrant
ratio phenomenon [ARPpath (1984) 22 7794]) characterized
by abnormal segregation ratios for one or more genetic markers.
hordeolum Syn. STYE.
horizontal resistance (plant pathol.) In a given cultivar: the
existence of similar levels of resistance to each of the races
of a given pathogen. Unlike VERTICAL RESISTANCE, horizontal
resistance tends to be a permanent (though not necessarily
complete) form of resistance which does not readily break down
when genetic changes occur in the pathogen; it is commonly
inherited polygenically.
horizontal transmission (lateral transmission) Transmission of a
disease or parasite from one individual to another contemporary
individual. (cf. VERTICAL TRANSMISSION.)
Hormidium Syn. KLEBSORMIDIUM.
Hormiscium dermatitidis See WANGIELLA.
Hormoconis A genus of fungi of the HYPHOMYCETES. H. resinae
(formerly Cladosporium resinae, the creosote fungus or
kerosene fungus) can utilize e.g. creosote and various hydrocarbons as sources of carbon (see also PETROLEUM). [Mechanism
of dodecane uptake by H. resinae: JGM (1986) 132 751756.]
The teleomorph of H. resinae is the ascomycete Amorphotheca
resinae. [Discussion and references on re-naming of C. resinae:
MS (1986) 3 169.]
hormocyst In certain cyanobacteria: short filaments composed
of granular cells surrounded by a common, condensed sheath
formed in intercalary or terminal positions in the vegetative trichome; hormocysts become detached from the parent trichome
and appear to function as propagules (cf. AKINETE and HORMOGONIUM). (See also LEMPHOLEMMA.)
Hormodendrum dermatitidis See WANGIELLA.
Hormodendrum resinae Syn. Hormoconis resinae.
hormogonium A short filament of undifferentiated cells (i.e.,
lacking heterocysts or akinetes) formed by filamentous CYANOBACTERIA (members of sections III, IV and V) and by e.g.
Beggiatoa; hormogonia may be formed by the fragmentation
of whole filaments (e.g. in Oscillatoria and Cylindrospermum)
or may develop from the tips of trichomes (e.g. in Scytonema).
(See also NECRIDIUM.) Hormogonia may differ from the parent
trichome e.g. in having smaller cells; they are typically motile
(by gliding) and usually move some distance before developing into mature filaments, thus functioning as propagules. In
some cyanobacteria (e.g. Nostoc muscorum [JGM (1983) 129
263270], Calothrix spp), GAS VACUOLES are formed only in
the hormogonia, the increased buoyancy they confer presumably
aiding in the dispersal of the hormogonia.
hormone A substance which is released from specialized cells in
specific part(s) of a multicellular organism and which, in small
quantities, can bring about one or more specific responses when
translocated to other part(s) of the same individual.
hot-spot
but is now referred to as parvovirus B19 or B19 parvovirus (see
ERYTHROVIRUS).)
HQNO HYDROXYQUINOLINE-N-OXIDE.
hr mutant HOST-RANGE MUTANT.
HR756 Syn. cefotaxime (see CEPHALOSPORINS).
Hrp secretion pathway (plant pathol.) See AVIRULENCE GENE.
HRP-2 protein See MALARIA.
HS HAEMOPHAGOCYTIC SYNDROME.
hybridization
Hungate technique See ROLL-TUBE TECHNIQUE.
Hungate tube A gas-tight, tube-shaped glass vessel with a rubber
stopper which is held in place by a screw cap; it is used in the
ROLL-TUBE TECHNIQUE.
hupA, hupB genes In Escherichia coli, the genes which encode
the two subunits of the HU PROTEIN.
Huroniospora See STROMATOLITES.
HUS See HAEMOLYTIC URAEMIC SYNDROME.
hut genes Genes involved in histidine utilization (see HISTIDINE
DEGRADATION).
Hutchinsons teeth See SYPHILIS.
HUVEC Human umbilical vascular endothelial cell.
HVR-1 (in hepatitis C virus) See HEPATITIS C VIRUS.
hyaline Transparent, translucent, or colourless.
hyaline cap See PSEUDOPODIUM.
hyalodendrins See EPIPOLYTHIAPIPERAZINEDIONES.
hyalodidymae See SACCARDOAN SYSTEM.
hyaloplasm (1) Syn. CYTOSOL. (2) See SARCODINA.
Hyalospora See UREDINIOMYCETES and AMPHISPORE.
Hyalotheca A genus of filamentous placoderm DESMIDS. The
filaments are composed of chains of cylindrical, flat-ended cells;
each cell has only a slight median constriction.
hyaluronan Syn. HYALURONIC ACID.
hyaluronate lyase (spreading factor; EC 4.2.2.1) A LYASE
which cleaves HYALURONIC ACID at the (1 4)-b-linkages; the
end product is a disaccharide containing a 4,5-unsaturated uronic
acid residue. (cf. HYALURONIDASE). It is produced e.g. by most
coagulase +ve staphylococci, Streptococcus pneumoniae, S. pyogenes and Clostridium perfringens ( toxin); it may promote
invasiveness. It can be assayed by its ability to reduce viscosity
in a solution of hyalauronic acid. [Action of enzyme from S.
pneumoniae: EMBO (2000) 19 12281240.]
hyaluronic acid A linear polysaccharide in which repeating disaccharide units of b-D-glucuronopyranosyl-(1 3)-N-acetyl-Dglucosamine are connected by (1 4)-b-linkages. Hyaluronic
acid occurs e.g. as an intercellular constituent of various animal
tissues, in synovial fluid, and in the capsules of certain group A
streptococci. Hyaluronic acid forms highly viscous solutions in
water and readily forms gels.
hyaluronidase Any enzyme which cleaves HYALURONIC ACID;
they include HYDROLASES and LYASES. The hydrolases include
hyaluronate 4-glucanhydrolase (EC 3.2.1.35) present e.g. in
testicular extracts and produced e.g. by certain streptomycetes.
The name hyaluronidase is often used (erroneously) as a
synonym for the enzyme HYALURONATE LYASE.
hybrid antibody See CONJUGATION (2).
hybrid-arrested translation A method for identifying a protein
encoded by a given cDNA. mRNAs from the cell are translated in the presence of cloned, single-stranded copies of the
cDNA. mRNAs which do not bind cDNA yield proteins incorporating a labelled amino acid. Translation is repeated without
cDNAs, allowing translation of the mRNA previously blocked
by hybridization to cDNA. The protein of interest is the extra
protein formed in the second translation.
hybrid plasmid (1) Any recombinant PLASMID (see e.g. CLONING).
(2) A recombinant plasmid containing sequences derived from
organisms which can normally exchange genetic information.
(cf. CHIMERIC PLASMID.)
hybridization (1) The formation of a double-stranded nucleic
acid by base-pairing between single-stranded nucleic acids
derived (usually) from different sources; some authors use the
term specifically for the association of ssRNA with ssDNA. (See
also DNA HOMOLOGY and SOUTHERN HYBRIDIZATION.)
hydrogen swell
and then an oxygen atom is introduced into the ring (forming a
lactone) by a cyclohexanone monooxygenase. The lactone can
then be hydrolysed to form a (non-cyclic) dicarboxylic acid.
Aromatic hydrocarbons (benzene, naphthalene, anthracene
etc) are present in e.g. petroleum and are formed by the incomplete combustion of almost any organic material; they are therefore common pollutants, and many are recognized carcinogens.
Bacteria (e.g. Pseudomonas spp) metabolize aromatic hydrocarbons by initially incorporating two atoms of oxygen into the
substrate to form a cis-dihydrodiol; the reaction is catalysed by
a multicomponent enzyme system comprising a dioxygenase, a
flavoprotein, and IRONSULPHUR PROTEINS. The cis-dihydrodiol is
oxidized to a catechol which is in turn a substrate for another
dioxygenase system which breaks open the aromatic ring. In contrast, fungi oxidize aromatic hydrocarbons using a cytochrome
P-450-dependent monooxygenase to form a reactive arene oxide;
this can either undergo isomerization to form a monohydric phenol, or enzymic hydrolysis to form a trans-dihydrodiol.
[Reviews on microbial hydrocarbon metabolism: Book ref.
155.]
Hydroclathrus See PHAEOPHYTA.
Hydrodictyon
A genus of freshwater green algae (division
CHLOROPHYTA) which form free-floating net-like colonies (water
nets) composed of large, coenocytic cells.
hydrogen (as a metabolite) Gaseous (molecular) hydrogen is produced e.g. in various types of FERMENTATION (sense 1), and is
formed during NITROGENASE activity. Gaseous hydrogen may be
consumed e.g. during METHANOGENESIS and may be used for
lithotrophic metabolism by e.g. HYDROGEN-OXIDIZING BACTERIA
and some SULPHATE-REDUCING BACTERIA. [Production and uptake
of molecular hydrogen by unicellular cyanobacteria: JGM (1985)
131 15611569.] (See also FORMATE HYDROGEN LYASE and
INTERSPECIES HYDROGEN TRANSFER.)
hydrogen bacteria Syn. HYDROGEN-OXIDIZING BACTERIA.
hydrogen dehydrogenase Syn. HYDROGENASE.
hydrogen hypothesis See EUKARYOTE.
hydrogen-oxidizing bacteria (the hydrogen bacteria; knallgas
bacteria) A phrase sometimes used to refer specifically to
a (non-taxonomic) category of aerobic bacteria which can
grow chemolithoautotrophically by obtaining energy from the
oxidation of gaseous hydrogen by oxygen via an electron
transport chain (see KNALLGAS REACTION); most species can
also grow chemoorganoheterotrophically and/or mixotrophically. [Details of the obligately chemolithoautotrophic hydrogenoxidizing species Hydrogenobacter thermophilus (gen. nov., sp.
nov.): IJSB (1984) 34 510.] The hydrogen-oxidizing bacteria, sensu stricto, are distinct from those bacteria which can
oxidize H2 without autotrophic CO2 fixation and/or which can
carry out anaerobic oxidation of H2 coupled to the reduction
of e.g. SO4 2 , CO2 or fumarate. The hydrogen-oxidizing bacteria (which include most or all CARBOXYDOBACTERIA) include
e.g. those strains of Alcaligenes denitrificans formerly called
A. ruhlandii ; Aquaspirillum autotrophicum; Bacillus schlegelii
[JGM (1979) 115 333341]; Paracoccus denitrificans; Pseudomonas facilis and P. saccharophila; and bacteria referred to
as Alcaligenes eutrophus, Nocardia autotrophica, and N. opaca.
Most hydrogen-oxidizing bacteria (including e.g. Paracoccus
denitrificans) have only a membrane-bound, NAD-independent
HYDROGENASE (see also EXTRACYTOPLASMIC OXIDATION); some
strains have only a soluble (cytoplasmic), NAD-reducing hydrogenase (hydrogen dehydrogenase), while others (e.g. strains of
Alcaligenes eutrophus) have both forms of the enzyme.
[Habitats, culture, and descriptions of individual hydrogenoxidizing bacteria: Book ref. 45, pp. 865893.]
hydrogenase
thus, e.g. prokaryotes occur in the gill cells of the giant clam
(Calyptogena magnifica) and in the TROPHOSOME tissue of the
giant tube worm, Riftia pachyptila. A living community at a
given vent appears to last for several years to several decades.
[Biology and microbiology of hydrothermal vents: Science
(1985) 229 713725; evidence for chemosynthetic primary
production in hydrothermal vents: Book ref. 202, pp. 319360.]
hydroxamates (in iron uptake) See SIDEROPHORES.
hydroxyapatite (hydroxylapatite; Ca10 (PO4 )6 (OH)2 ) A mineral
which is used as a stationary phase in adsorption CHROMATOGRAPHY e.g. for separating ssDNA from dsDNA or RNA. Under
certain ionic conditions the mineral adsorbs dsDNA; the dsDNA
is desorbed at higher ionic concentrations.
hydroxycobalamin See VITAMIN B12 .
hydroxyethylcellulose See HE-CELLULOSE.
hydroxyl radical (OH or OH) A hyper-reactive radical formed
e.g. during a reaction involving SUPEROXIDE and HYDROGEN
PEROXIDE (the HaberWeiss reaction); this reaction can be
catalysed by iron complexes (e.g. FeEDTA, Fetransferrin)
and may be represented in two phases: (i) the reduction of ferric
(with the formation of ferrous complexes and
complexes by O
2
SINGLET OXYGEN), and (ii) the oxidation of ferrous complexes
by H2 O2 (with the formation of ferric complexes, OH and
OH) [FEBS (1978) 86 139142]. (Hydroxyl radical is also
reported to be formed e.g. in a reaction involving superoxide
and hypochlorite, and by the action of ultraviolet radiation
on hydrogen peroxide.) During PHAGOCYTOSIS, LACTOFERRIN
from activated NEUTROPHILS may catalyse the formation of
OH, thus enhancing antimicrobial activity. Scavengers of OH
used in experimental systems include e.g. benzoate, dimethyl
sulphoxide, mannitol and salicylate.
hydroxylamine (as a MUTAGEN) Hydroxylamine (NH2 OH) reacts
mainly with cytosine residues (and, much more slowly, with
adenine residues) in DNA (particularly ssDNA), replacing the
amino group with a hydroxyamino group (NHOH); this
favours tautomerization of the base such that, during subsequent
DNA replication, mispairing occurs (resulting predominantly in
GC to AT transitions). Although hydroxylamine is an effective
mutagen when used to treat certain viruses or e.g. transforming
DNA, any mutagenic effect it may have in living cells is
generally masked by its toxic or lethal effects. The related
compound methoxyamine (NH2 OCH3 ) acts in a similar way.
hydroxylapatite Syn. HYDROXYAPATITE.
hydroxylase Syn. MONOOXYGENASE.
hydroxymethionine analogue See HMA.
6-(p-hydroxyphenylazo)uracil See HPURA.
hydroxypyrimidine antifungal agents A group of agricultural
systemic ANTIFUNGAL AGENTS which have a highly selective
action against powdery mildews; resistance to these fungicides
tends to develop rapidly. Hydroxypyrimidines include e.g.
DIMETHIRIMOL and ETHIRIMOL.
8-hydroxyquinoline (oxine; 8-quinolinol) (as antimicrobial agent)
A chelating agent which, in the presence of Cu2+ or Fe2+ ,
has antifungal and antibacterial activity; Gram-positive bacteria
are much more susceptible than Gram-negative bacteria. The
potentiating effects of Cu2+ and Fe2+ are antagonized by trace
amounts of Co2+ , while Ni2+ acts as a competitive inhibitor.
COPPER oxine has been used in agricultural antifungal sprays and
as a rot-proofing agent for e.g. textiles.
Some halogenated derivatives of oxine are used e.g. for the
treatment or prophylaxis of amoebic dysentery. They include
hypha
hypericin See STENTORIN.
hyper-IgM syndrome See RNA EDITING.
hyperimmune Refers to the condition of an individual whose
plasma contains a high titre of a particular antibody following
repeated exposure of the individual to the homologous antigen.
Hyperimmune serum is serum derived from such an individual.
Hypermastigida An order of protozoa (class ZOOMASTIGOPHOREA)
which have numerous flagella, the kinetosomes being arranged
in complete or incomplete circles; the organisms are associated
with insects. Genera: e.g. Barbulanympha, Lophomonas, Microjoenia, Spirotrichonympha, TRICHONYMPHA.
hyperparasite A parasite of a parasite.
hyperplasia The enlargement of an organ or tissue owing to an
increase in the number of cells. (Hence adj. hyperplastic.) (cf.
HYPERTROPHY and NEOPLASIA.)
hypersensitivity (1) (immunol.) The state of a PRIMED individual who, on further exposure to the relevant antigen, gives
an exaggerated immune response that causes varying degrees
of harm ranging from a mild local inflammatory reaction to
death. (See IMMEDIATE HYPERSENSITIVITY and DELAYED HYPERSENSITIVITY; see also BRUCELLOSIS.)
(2) (plant pathol.) The expression of extreme reactivity by
a plant in response to a potential parasite or pathogen, the
plants response commonly serving to limit or prevent parasitization/disease. Hypersensitivity typically involves rapid cell death
at the (localized) site of infection and the concomitant induction of e.g. PHYTOALEXIN(s) by microbial elicitors; the induction
of phytoalexins by microbial elicitors involves the expression
of new host genes and the formation of new species of mRNA
and new enzymes. (In addition to phytoalexin production, microbial elicitors can also apparently e.g. stimulate the formation of
ETHYLENE and bring about the accumulation of LIGNIN.) (See also
PATHOGENESIS-RELATED PROTEINS.) In many cases the combination
of cell death and accumulation of phytoalexin(s) at the site of
infection appears to provide the level of resistance needed to prevent disease development. When the challenging microorganism
is an obligate parasite (i.e., a BIOTROPH), the death of host cells
may, in itself, be sufficient to prevent the spread of the parasite
to uninfected tissues.
hypersensitivity pneumonitis Syn. EXTRINSIC ALLERGIC ALVEOLITIS.
hypertrophy Enlargement of an organ or tissue owing to an
increase in the size of pre-existing cells. (cf. HYPERPLASIA.)
hypervariable region (immunol.) Any of several amino acid
sequences, located in the VARIABLE REGIONS of the heavy chain
and light chain of IMMUNOGLOBULINS, which exhibits a degree of
variability (in composition) greater than that found in other parts
of the variable region. (See also COMPLEMENTARITY-DETERMINING
REGIONS.)
hypha (pl. hyphae) (1) (bacteriol., mycol.) In many (mycelial)
fungi and in some bacteria (see ACTINOMYCETALES): a branched
or unbranched filament, many of which together constitute the
vegetative form of the organism and (in some species) form the
sterile portion of a fruiting body; a mass of vegetative hyphae
is referred to as a MYCELIUM.
Fungal hyphae. Each hypha has a tubular CELL WALL which,
in many species, is divided into compartments or cells by crosswalls (see SEPTUM (b)); in both septate and aseptate species,
the cell wall is external to the CYTOPLASMIC MEMBRANE which
encloses the cytoplasm, NUCLEUS or nuclei, and other components typical of eukaryotic organization. (See also VACUOLE.)
The diameter of a hypha ranges from about 1 m to macroscopic
dimensions, depending e.g. on species. Hyphae grow mainly by
apical extension see GROWTH (fungal).
7-iodo-8-hydroxyquinoline-5-sulphonate (chiniofon); 5,7-diiodo8-hydroxyquinoline (diiodohydroxyquin; Diodoquin); 5-chloro7-iodo-8-hydroxyquinoline (iodochlorohydroxyquin; Enterovioform; Vioform). (Some of these derivatives also have useful
antibacterial and antifungal properties.)
hydroxyquinoline-N-oxide (HOQNO; HQNO) 2-Alkyl-4-hydroxyquinoline-N-oxides (e.g. 2-n-heptyl-4-HOQNO) act as RESPIRATORY INHIBITORS in mitochondria and in certain bacteria some
bacteria are apparently impermeable to HOQNOs; HOQNOs
appear to resemble ANTIMYCIN A (q.v.) in their mode of action.
HOQNOs also inhibit the Na+ pump in Vibrio alginolyticus (see
SODIUM MOTIVE FORCE).
2-hydroxystilbamidine An aromatic DIAMIDINE which has trypanocidal and antifungal activity; it has been used e.g. in the
treatment of blastomycosis and African trypanosomiasis.
5-hydroxytryptamine Syn. SEROTONIN.
hydroxyurea (HU; HONH.CO.NH2 ) A reagent which prevents
the synthesis of deoxyriboNUCLEOTIDES by specifically inhibiting
ribonucleoside diphosphate reductase.
Hyella See PLEUROCAPSA GROUP.
Hygrocybe See AGARICALES (Hygrophoraceae).
hygromycin B An AMINOGLYCOSIDE ANTIBIOTIC which, like STREPTOMYCIN, appears to act at a single ribosomal site.
hygrophilic (hygrophilous) Requiring a moist habitat for optimum growth.
Hygrophoraceae See AGARICALES.
Hygrophorus See AGARICALES (Hygrophoraceae).
hymenium (mycol.) A layer of ascospore- or basidiosporeforming tissue e.g. that lining an APOTHECIUM or that forming
the surface of a LAMELLA; a hymenium may also contain sterile
structures see e.g. PARAPHYSIS and PSEUDOPARAPHYSIS.
Hymenochaetaceae See APHYLLOPHORALES.
Hymenochaete See APHYLLOPHORALES (Hymenochaetaceae).
Hymenogaster See GASTEROMYCETES (Hymenogastrales).
Hymenogastrales See GASTEROMYCETES.
Hymenomonas See COCCOLITHOPHORIDS.
Hymenomycetes A class of fungi (subdivision BASIDIOMYCOTINA)
in which the typical fruiting body is a well-developed, macroscopic, gymnocarpous or semiangiocarpous structure containing BALLISTOSPORE-bearing basidia in a HYMENIUM. Subclasses:
HOLOBASIDIOMYCETIDAE and PHRAGMOBASIDIOMYCETIDAE.
hymenophore That part of a fruiting body which bears a
HYMENIUM or SUBHYMENIUM, or the entire (hymenium-bearing)
fruiting body. (cf. SPOROPHORE.)
Hymenostomatia A subclass of (mostly) freshwater ciliates
(class OLIGOHYMENOPHOREA) in which somatic ciliature is often
uniform, the buccal cavity (when present) is ventral, and
kinetodesmata are usually conspicuous; sedentary and colonial
types are not common. Orders: ASTOMATIDA, HYMENOSTOMATIDA,
SCUTICOCILIATIDA.
Hymenostomatida An order of protozoa (subclass HYMENOSTOMATIA) in which the buccal cavity is well defined and contains
characteristic membranelles. A SCUTICA does not appear during
stomatogenesis. Genera (which may be distinguished e.g. by the
number of post-oral kineties) include e.g. COLPIDIUM, Frontonia, GLAUCOMA, ICHTHYOPHTHIRIUS, LAMBORNELLA, Ophryoglena,
PARAMECIUM and TETRAHYMENA.
hyperauxinic Containing or producing abnormally high levels of
AUXINS.
hyperchromic shift A change in the amount of ultraviolet
radiation absorbed by a nucleic acid during changes from the
double-stranded to the single-stranded condition, or vice versa
(see e.g. THERMAL MELTING PROFILE).
381
hyphal body
In basidiomycetes the primary hyphae are uninucleate haploid hyphae which develop when basidiospores germinate; the
secondary (dikaryotic) hyphae develop following DIKARYOTIZATION.
A basidiocarp may, according to species, consist of one, two
or three distinct types of hypha corresponding, respectively, to
a monomitic, dimitic or trimitic sporocarp. A monomitic sporocarp contains only generative hyphae: typically thin-walled,
branched, septate hyphae which give rise to basidia; generative hyphae may contain CLAMP CONNECTIONS if the organism
normally forms clamps on its vegetative mycelium. A dimitic
sporocarp contains generative hyphae together with either skeletal hyphae or binding hyphae (both of which originate from
generative hyphae). Skeletal hyphae are typically thick-walled
and unbranched; they are sterile (i.e., do not form basidia) and
do not form clamps. Binding (= ligative) hyphae are sterile,
highly branched, and do not form clamps; in trimitic sporocarps
they bind together the generative and skeletal hyphae.
(2) (bacteriol.) See PROSTHECA.
hyphal body In some species of the ENTOMOPHTHORALES: a piece
of fragmented mycelium which can germinate to form a sporebearing structure.
hyphenated dyad symmetry See e.g. PALINDROMIC SEQUENCE.
Hyphochytriaceae See HYPHOCHYTRIOMYCETES.
Hyphochytriales See HYPHOCHYTRIOMYCETES.
Hyphochytridiomycetes See HYPHOCHYTRIOMYCETES.
Hyphochytriomycetes A class of fungi (subdivision MASTIGOMYCOTINA) which form zoospores having one anteriorly-directed
tinsel flagellum. The organisms include terrestrial species as well
as aquatic saprotrophs and parasites of other fungi and of freshwater and marine algae; they closely resemble members of the
CHYTRIDIALES in morphology and life cycle, but they apparently
do not carry out sexual processes. One order: Hyphochytriales;
three families: Anisolpidiaceae, Hyphochytriaceae and Rhizidiomycetaceae (e.g. RHIZIDIOMYCES).
This class has been called Hyphochytridiomycetes by many
authors. [Validation of the name Hyphochytriomycetes: Book
ref. 174, p. 285.]
Hypholoma See AGARICALES (Strophariaceae).
Hyphomicrobium A genus of PROSTHECATE BACTERIA found in
soils and in freshwater, estuarine and marine habitats. Morphologically, Hyphomicrobium resembles RHODOMICROBIUM, and
its cell cycle is very similar to the simplified cell cycle of
R. vannielii ; it differs from R. vannielii e.g. in the absence
of pigments and in that its swarm cells bear a single subpolar flagellum. (Phages specific for developing daughter cells
have been isolated [JGV (1979) 43 2938].) The organisms are
chemoorganotrophs which can use one-carbon compounds (e.g.
methanol, methylamine) as sole sources of carbon and energy
(see METHYLOTROPHY); one-carbon compounds are metabolized
via the icl serine pathway. Growth occurs either aerobically
or anaerobically with nitrate (which is reduced to nitrogen
via nitrite); optimum growth temperature: 2530 C. GC%: ca.
5967. [Review: ARM (1981) 35 567594.]
Hyphomonas A genus of Gram-negative, aerobic, asporogenous,
non-photosynthetic, heterotrophic, PROSTHECATE BACTERIA which
reproduce by budding; daughter cells are motile (swarm cells),
having one or more flagella according to species. The cell body
may vary in size and shape during the cell cycle, and usually
has a single polar prostheca (hypha). Iron and manganese
salts are not deposited on the cell surface (cf. PEDOMICROBIUM).
Amino acids are the preferred substrates for growth; onecarbon compounds are not used (cf. HYPHOMICROBIUM). Species:
Hyuga fever
sodium hypochlorite solutions are often stabilized with sodium
hydroxide. Sodium hypochlorite is used in a range of
DISINFECTANTS and bleaches (e.g. Chloros, Domestos, Milton).
Aerosols of hypochlorite solutions have been used for the
disinfection of air. (N.B. Hypochlorite solutions react with
formaldehyde to form the carcinogen bis-chloromethylether.)
(See also DICHLOROISOCYANURATE.)
hypocone See DINOFLAGELLATES.
Hypocrea See HYPOCREALES.
Hypocreales An order of mainly saprotrophic, plant-parasitic or
fungicolous fungi of the subdivision ASCOMYCOTINA; anamorphs
occur e.g. in the genera ACREMONIUM, CYLINDROCARPON and
FUSARIUM. Ascocarp: perithecioid or closed, frequently on or
within a stroma and often brightly coloured. Asci: cylindrical to
clavate. Ascospores: usually colourless, aseptate to multiseptate
or muriform. Some genera in the order have traditionally been
distinguished on the basis of the number of septa in their
ascospores; spore septation has not been recognized as a valid
taxonomic criterion [Mycol. Pap. (1983) Nr 150 ]. Genera: e.g.
Calonectria, GIBBERELLA, Hypocrea, NECTRIA.
Hypocrella See CLAVICIPITALES.
Hypoderma See RHYTISMATALES.
hypogean Occuring underground (cf. EPIGEAN).
Hypogymnia A genus of LICHENS (order LECANORALES). The thallus is foliose, with often hollow, inflated lobes, grey to greyishbrown above, black beneath; rhizines are absent. H. physodes is
very common e.g. in the UK; it is tolerant of air pollution and
is often the only macrolichen to be found in and around towns
and cities.
hypolimnion In a lake: the layer of water between the METALIMNION and the lake bottom; characteristically, it is anaerobic
and rich in sulphide.
Hypomyces A genus of mainly fungicolous fungi of the order
CLAVICIPITALES; anamorph: Cladobotryum. (See also COBWEB
DISEASE.)
hyponeuston See NEUSTON.
hypophloeodal Syn. ENDOPHLOEODAL.
Hypopylaria A category (section) of LEISHMANIA species which
develop in the midgut and hindgut of the arthropod vector; it
includes L. agamae and L. ceramodactyli . (cf. PERIPYLARIA,
SUPRAPYLARIA.)
hyposensitization (immunol.) Syn. DESENSITIZATION.
Hyposoter exiguae virus See POLYDNAVIRIDAE.
hypostatic allele See EPISTASIS.
Hypostomatia A subclass of ciliates (class KINETOFRAGMINOPHOREA) in which the cytostome (when present) generally
occurs on the ventral surface, and the cytopharyngeal apparatus
is of the CYRTOS type; the body is typically cylindrical or
dorsoventrally flattened, and the somatic ciliature is often
reduced. The orders are:
Apostomatida. Cytostome inconspicuous or absent; rosette
(secretory organelle?) commonly present in the oral area;
somatic ciliature spirally arranged in mature organisms; cysts
common (see also TOMITE); often associated with marine
383
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
I
I Isoleucine (see AMINO ACIDS).
(I + C + D) model Syn. HELMSTETTERCOOPER MODEL.
I-like pili See PILI.
I period See HELMSTETTERCOOPER MODEL.
Ia antigens Class II antigens of the murine MAJOR HISTOCOMPATIBILITY COMPLEX. (See also IR GENES.)
Ia protein The Escherichia coli OmpF PORIN.
IAA Indole 3-acetic acid (see AUXINS).
IAEA International Atomic Energy Agency.
IAHS Infection-associated haemophagocytic syndrome: see
HAEMOPHAGOCYTIC SYNDROME.
IAM Institute of Applied Microbiology, University of Tokyo,
Yayoi, Bunko-Ku, Tokyo, Japan.
IAP Intracisternal A-TYPE PARTICLE.
iatrogenic Refers to any disease or infection which is caused
or exacerbated, unintentionally, as a result of medical intervention e.g. examination or treatment.
IAVI International AIDS Vaccine Initiative.
Ib protein The Escherichia coli OmpC PORIN.
ibotenic acid See AMATOXINS.
IBV Infectious bronchitis virus (CORONAVIRIDAE).
ICAD See APOPTOSIS.
ICAM-1 Syn. CD54.
ICAM-2 See CD102.
ICAM-3 See IMMUNOGLOBULIN SUPERFAMILY.
ICDH Isocitrate dehydrogenase: see TCA CYCLE.
ICE (syn. caspase-1) See APOPTOSIS.
ice algae See DIATOMS.
ice nucleation bacteria Those bacteria which, at temperatures just below 0 C, promote water-to-ice transition by acting as nuclei around which ice crystals can form. Such
bacteria (e.g. strains of Erwinia herbicola, Pseudomonas fluorescens, P. syringae and Xanthomonas campestris) which
include some common epiphytes have been implicated as contributory factors in frost damage in various agricultural crops.
A DNA fragment from P. fluorescens, when cloned in
Escherichia coli, can confer the ice-nucleation phenotype; the
fragment may encode an OUTER MEMBRANE protein of MWt ca.
180000 [EMBO (1986) 5 231236]. When grown at 15 C, most
ice-nucleation-positive strains of Erwinia herbicola shed into
the medium vesicles composed of outer membrane; these vesicles (cell-free ice nuclei) can behave as ice-nucleation centres
which are active at 2 C to 10 C [JB (1986) 167 496502].
Some plant tissues survive, without damage, when supercooled to several degrees below 0 C but may suffer frost
damage if ice-nucleation bacteria are present. Above (approx.)
5 C, the incidence of frost injury can be decreased by reducing
the size of the populations of plant-contaminating ice-nucleation
bacteria. This can be done e.g. by treatment of plant surfaces
with antibiotics such as streptomycin or oxytetracycline; an alternative method is to treat plant surfaces with non-ice-nucleating
bacteria (a form of BIOLOGICAL CONTROL). A combination of
antibiotic treatment and biological control has been found to act
additively in the control of frost injury in pear trees [Phytopathol.
(1996) 86 841848].
Iceland moss See CETRARIA.
ich See ICHTHYOPHTHIRIASIS.
ichthyo- Prefix denoting fish e.g. ichthyopathology: the study
of FISH DISEASES; ichthyotoxic: toxic to fish.
IgA1 proteases
IDAV See HIV.
idiogram See KARYOTYPE.
idiolite A product of SECONDARY METABOLISM.
idiopathic (of a disease) Of unknown cause.
idiophase In BATCH CULTURE, that phase in which SECONDARY
METABOLISM is dominant (cf. TROPHOPHASE); it corresponds to
the latter part of the log phase together with the stationary phase.
idiosome (protozool.) See XENOSOME (2).
idiotope See IDIOTYPE.
idiotype An Ig molecule defined by the sum total of antigenic
determinants (idiotopes) on its variable (VH and/or VL ) domains.
idli A type of steamed bread from India. It is made from a
batter of milled rice and black gram (Phaseolus mungo) which
is left to ferment overnight. The fermentation is carried out
mainly by Leuconostoc mesenteroides which produces acid
and gas; Enterococcus faecalis, and sometimes Pediococcus
cerevisiae, contribute acidity, and yeasts may also be involved.
The leavened batter is then steamed.
idling During DNA replication: repeated cycles of addition and
excision of nuleotides at a 3 terminal with no net synthesis or
degradation of DNA. [Idling as a mechanism in lagging strand
synthesis: GD (2004) 18 27642773.]
idoxuridine (IDU; 5-iodo-2 -deoxyuridine; IUdR) An ANTIVIRAL
AGENT which acts as an analogue of thymidine (5-methyl-2 deoxyuridine). Selective toxicity is poor, and the drug is too
toxic for systemic use; it may be used topically for the treatment
of e.g. herpes simplex keratitis, but is being superseded by more
recent antiviral drugs.
IDU IDOXURIDINE.
IEF ISOELECTRIC FOCUSING.
IEM IMMUNOELECTRON MICROSCOPY.
IEP (1) ISOELECTRIC POINT. (2) IMMUNOELECTROPHORESIS.
IF INTERMEDIATE FILAMENT.
IF-1, IF-2, IF-3 See PROTEIN SYNTHESIS.
IF1 protein See PROTON ATPASE.
IFA test Syn. IFAT.
IFAT See indirect IMMUNOFLUORESCENCE.
IFN INTERFERON.
IFO Institute for Fermentation, 1785 Juso-Honmachi, 2-Chome,
Yodogawa-Ku, Osaka, Japan.
IFT Syn. IFAT.
Ig IMMUNOGLOBULIN.
IgA Immunoglobulin A, the predominant IMMUNOGLOBULIN in
saliva, tears, colostrum and other body fluids, but comprising
only ca. 10% of the total plasma Igs. The IgA monomer (MWt
ca. 160000; S20
W 7) contains alpha HEAVY CHAINS, kappa or
lambda LIGHT CHAINS, and ca. 8% carbohydrate. Most IgA at
mucosal surfaces (secretory IgA, sIgA, SIgA) is in dimeric form:
two monomers are linked via a J CHAIN, and the whole is linked to
the SECRETORY COMPONENT. Polymers larger than dimers are also
formed. IgA can fix complement via the alternative pathway.
There are two subclasses: IgA1 and IgA2. (See also entry IgA1
proteases.)
IgA1 proteases Various extracellular bacterial enzymes which
specifically cleave the human IgA1 antibody at the heavychain hinge region but which do not affect IgA2; some are
sensitive to EDTA. These enzymes are synthesized by e.g.
Haemophilus influenzae, Neisseria gonorrhoeae, N. meningitidis
and Streptococcus pneumoniae bacteria which are typically
pathogenic at or via the mucosal surfaces; presumably, IgA1
proteases counteract the hosts IgA1 defences, but the role of
these enzymes in pathogenesis has not been established.
At least some IgA1 proteases are secreted by a type IV system
(see PROTEIN SECRETION).
IgD
IgD Immunoglobulin D, an IMMUNOGLOBULIN present in very low
concentrations in plasma; it occurs mainly as a surface receptor
for antigen on the membranes of B LYMPHOCYTES. The IgD
molecule (MWt ca. 175000; S20
W 7) contains delta HEAVY CHAINS,
kappa or lambda LIGHT CHAINS, and ca. 1213% carbohydrate.
IgE Immunoglobulin E, an IMMUNOGLOBULIN found in minute
quantities in plasma. The IgE molecule (MWt ca. 190000; S20
W 8)
contains epsilon HEAVY CHAINS, kappa or lambda LIGHT CHAINS,
and ca. 12% carbohydrate. IgE binds to basophils and mast
cells via its Fc portion, causing degranulation in the presence of
specific allergen and thus effecting a TYPE I REACTION; cytophilic
activity is abolished e.g. by heating (56 C/34 hours).
IgG Immunoglobulin G, the predominant IMMUNOGLOBULIN in
plasma (ca. 916 mg/ml, 75% of total plasma Ig). The IgG
molecule (MWt ca. 150000; S20
W 7) contains gamma HEAVY
CHAINS, kappa or lambda LIGHT CHAINS, and ca. 3% carbohydrate. There are four subclasses IgG1, IgG2, IgG3 and
IgG4 distinguished by differences in amino acid sequences
and by serology; human IgG subclasses are numbered in order
of their concentrations in plasma: IgG1 comprises ca. 65% of
plasma IgG. IgG1 and IgG3 are bivalent COMPLEMENT-FIXING
ANTIBODIES (half-life ca. 21 and 7 days, respectively) which
are important e.g. as opsonins and antitoxins in extravascular
regions as well as in the bloodstream; in humans, they can
cross the placenta and are important in the protection of the
fetus and neonate. (Efficient binding of complement component
C1 appears to require an IgG doublet, i.e. two molecules side
by side; a single IgG molecule binds C1 only weakly.) IgG
antibodies generally appear to predominate in the secondary
(anamnestic) humoral reponse to antigen. (See also ALLOTYPE.)
IgG protease See e.g. ELASTASE.
IgM (macroglobulin) Immunoglobulin M, a minor plasma
IMMUNOGLOBULIN (comprising ca. 510% of total plasma Ig);
phylogenetically, IgM is apparently the most primitive class
of Igs. The IgM monomer (MWt ca. 180000) contains mu
HEAVY CHAINS, kappa or lambda LIGHT CHAINS, and ca. 12%
carbohydrate; monomeric IgM occurs as a surface receptor for
antigen on the B LYMPHOCYTE membrane. The typical form
of IgM is a pentamer (S20
W 19) in which the five monomers
are arranged radially (Fc portions directed towards the centre)
and connected via disulphide bonds, with a J CHAIN at the
centre of the polymer; in the free (uncombined) form, an
IgM antibody is therefore stellate, but pentameric IgM is
sufficiently flexible to assume a spider-like conformation in
order to combine with multiple-repeating antigens on a surface.
(IgM antibodies are thus particularly good agglutinators of those
antigens, e.g. bacteria, which display a pattern of repeated
antigenic determinants.) IgM antibodies are COMPLEMENT-FIXING
ANTIBODIES with a theoretical valency of 10. Maximum valency
is generally exerted only with small haptens; with larger antigens
the effective valency is often only 5. (It appears that an IgM
antibody must bind antigen at more than one of its combining
sites in order to be able to fix complement [Mol.Immunol. (1981)
18 863868, cited in Book ref. 42, p. 647].) In man, IgM does
not pass through blood vessel walls into the tissues, and does not
cross the placenta; its half-life is ca. 5 days. IgM antibodies are
often the first to be formed in the humoral response to antigen;
the humoral response to THYMUS-INDEPENDENT ANTIGENS (such
as purified pneumococcal polysaccharides) generally involves,
almost exclusively, the formation of IgM antibodies. The
Wassermann antibody (see WASSERMANN REACTION) and the
rheumatoid factor (see RHEUMATOID ARTHRITIS) are largely or
exclusively IgM antibodies.
IGS (mol. biol.) Internal guide sequence: see SPLIT GENE (b).
IHF INTEGRATION HOST FACTOR.
IkBa See CYTOKINES.
IL Abbreviation for interleukin. See separate entries for INTERLEUKIN-1 (IL-1), INTERLEUKIN-2 (IL-2) etc.
IL-1 INTERLEUKIN-1.
IL-1g Syn. INTERLEUKIN-18.
IL-2 INTERLEUKIN-2.
ilarviruses (isometric labile ringspot viruses; tobacco streak
virus group) A group of tripartite ssRNA-containing PLANT
VIRUSES which have a wide host range; transmission occurs
via seeds and pollen and can readily occur mechanically. Type
member: tobacco streak virus; other members include e.g. apple
mosaic virus, Citrus leaf rugose virus, Citrus variegation virus,
Prunus necrotic ringspot virus, spinach latent virus, Tulare apple
mosaic virus.
Virions: quasi-isometric, occasionally bacilliform; several
types occur, differing in size (ca. 2635 nm diam.) and in S20
W.
Genome: three molecules of linear positive-sense ssRNA: RNA1
(MWt ca. 1.1 106 ), RNA2 (MWt ca. 0.9 106 ) and RNA3
(MWt ca. 0.7 106 ); the coat protein mRNA (RNA4) is also
encapsidated. RNAs 1, 2 and 3, together with coat protein or
RNA4, are required for infectivity (cf. ALFALFA MOSAIC VIRUS).
ileocaecal syndrome Syn. NEUTROPENIC ENTEROCOLITIS.
Ilheus virus See FLAVIVIRIDAE.
illegitimate name In NOMENCLATURE: a validly published name
which contravenes any rule(s) of the relevant nomenclatural code.
illegitimate recombination Fortuitous RECOMBINATION which
occurs between DNA sequences which are non-homologous or
which have very short regions of homology. In Escherichia
coli illegitimate recombination is recA-independent and may be
mediated by GYRASE: strands cleaved during gyrase action at
different sites may undergo crossing over by the exchange of
gyrase subunits covalently bound to the cut ends [model: PNAS
(1983) 80 24522456].
imazalil An agricultural systemic ANTIFUNGAL AGENT, an imidazolyl derivative which acts as an inhibitor of sterol
biosynthesis, thereby disrupting the cytoplasmic membrane in
susceptible fungi. Imazalil is used mixed with e.g. guazatine
or thiophanate-methyl as a seed treatment against many seedborne pathogens of cereals (e.g. Ustilago and Pyrenophora spp).
It is also effective against Penicillium diseases of citrus fruits.
imbricated Overlapping, like tiles on a roof.
ImD unit See MICROCOMPLEMENT FIXATION.
IMF INTERMEDIATE FILAMENT.
imf phosphorylation See ELECTRON TRANSPORT PHOSPHORYLATION.
Imhoff tank A large tank formerly widely used for SEWAGE
TREATMENT. Essentially, crude sewage flows into a sludge
settlement chamber located within a larger tank; sludge falls
from a slot in the settlement chamber into the main digester
compartment where it undergoes ANAEROBIC DIGESTION. The tank
is vented for the escape of gases.
IMI Imperial Mycological Institute, the former name of the
Commonwealth Mycological Institute, Kew, UK.
imidazole antifungal agents See AZOLE ANTIFUNGAL AGENTS.
imipenem See THIENAMYCIN.
immediate hypersensitivity (immunol.) HYPERSENSITIVITY mediated by humoral antibodies: see TYPE I REACTION, TYPE II
REACTION, TYPE III REACTION, TYPE V REACTION (cf. DELAYED
HYPERSENSITIVITY). Immediate hypersensitivity reactions typically occur within minutes or hours of contact with specific
386
immune globulin
and labour of preparing purified immobilized enzymes. Cells can
be immobilized by the methods used for enzymes (see above),
but entrapment is the most commonly used method; gels used
include e.g. agar, alginate, k-carrageenan, polyacrylamide, and
polyurethane. Dead cells may be used for simple one-step or
two-step reactions (provided they retain specific enzymic activity), but living cells are necessary for multistep transformations
in which several enzymes act sequentially and/or in which there
is a need for the regeneration of cofactors. Examples of the
industrial use of dead immobilized cells include e.g. Escherichia
coli in a k-carrageenan gel for the production of L-aspartic
acid from ammonium fumarate, and Brevibacterium flavum
in a k-carrageenan gel for the production of L-malic acid from
fumaric acid. High cell densities can be achieved with immobilized living cells. Thus, e.g., in one process used for the production of ethanol, Saccharomyces cerevisiae (S. carlsbergensis)
is immobilized in carrageenan, and beads of the gel (containing
3.5 106 cells/ml) are incubated in a shaken nutrient medium
for 60 hours: cell density rises to over 5 109 cells/ml ca.
10 times higher than that possible in a conventional broth culture with the yeast cells densely packed within the surface
layer of each bead. When such beads are packed into a column and fed with a glucose-containing nutrient medium they
produce ethanol efficiently for long periods of time. Other uses
of immobilized living cells include the production of hydrogen
from cells of Anabaena cylindrica bound to glass beads, and
the production of an extracellular a-amylase by Bacillus subtilis
immobilized in a polyacrylamide gel.
[Book ref. 3, pp. 203222, and PTRSLB (1983) 300 369389
(cells); Book ref. 31, pp. 331367 (enzymes); Science (1983)
219 722727.]
(2) The inhibition of MOTILITY in a microorganism e.g. by
a specific antiserum (see IMMOBILIZATION TEST).
immobilization test Any test which involves the inhibition of
MOTILITY in a microorganism. Immobilization tests can be used
e.g. to detect specific antibodies (see e.g. TPI TEST) or organisms
(e.g. a given strain of Vibrio cholerae may be identified by
determining which types of specific antibody inhibit its motility).
Antibodies may immobilize a motile organism e.g. by mediating
the adhesion of flagella, or by promoting IMMUNE CYTOLYSIS.
immune (1) (adj.) Refers to the state of IMMUNITY (sense 2 or
3). (2) (noun) See EPIDEMIOLOGY.
immune adherence A phenomenon in which antigenantibody
complexes that have triggered COMPLEMENT FIXATION adhere
firmly to receptors on phagocytes; the enhanced adhesion
(which adds to that due to direct antigenantibodyphagocyte
interaction) is due mainly to component C3b.
The phrase immune adherence is sometimes used also
to refer to the totality of pathogenphagocyte adherence, i.e.
including both antibody-mediated and complement-mediated
adhesion.
immune complex An antigenantibody complex. Small, soluble
(i.e. non-precipitating) immune complexes are formed e.g. under
ANTIGEN EXCESS conditions. (See also TYPE III REACTION.)
immune cytolysis The lysis of a cell which has been sensitized
(SENSITIZATION sense 3) and which has triggered COMPLEMENT
FIXATION; lysis may result directly or indirectly from the formation of a pore, in the membrane, created by the membrane attack
complex. (cf. REACTIVE LYSIS.)
immune deficiency-associated virus See AIDS.
immune electron microscopy IMMUNOELECTRON MICROSCOPY.
immune globulin Antiserum (or its immunoglobulin fraction)
containing antibodies to a particular antigen or antigens.
antigen; they are also referred to as immediate-type hypersensitivity reactions to include those which require hours or days to
develop.
immediate-type hypersensitivity See IMMEDIATE HYPERSENSITIVITY.
Immedium filter See SEWAGE TREATMENT.
immersion lens See RESOLVING POWER.
immersion oil Cedarwood or synthetic oil (refractive index ca.
1.5) used with oil-immersion objectives (see RESOLVING POWER).
In homogeneous immersion the immersion oil, objective lens,
and cover-glass all have the same refractive index. Oil should be
removed from the objective with a lens tissue immediately after
use; unless otherwise recommended, a suitable solvent is 1,1,1trichloroethane, but benzene or xylene can be used. Prolonged
contact with solvents may damage lens mountings.
immobilization (1) (biotechnol.) Microbial, plant or animal cells,
or macromolecules, may be immobilized by attachment to solid
structures, incorporation in gels etc for use in e.g. BIOCONVERSIONS (sense 1) in some cases on an industrial scale. Various
immobilized macromolecules are used e.g. in procedures involving affinity CHROMATOGRAPHY.
Enzymes are immobilized because soluble enzymes are difficult to separate from substrates or products (and, hence, cannot
be re-used in industrial processes), and most are unstable under
conditions of use. The main methods of enzyme immobilization are: (a) Binding to a solid carrier or support. Supports
used for covalent binding include e.g. cellulose, ceramic, glass,
steel and synthetic polymers; usually, the support is activated
(see e.g. CYANOGEN BROMIDE), and the enzyme is then allowed
to bind (commonly via its amino or carboxyl groups) to the
activated support. The active site of the enzyme can be protected by allowing binding to occur in the presence of the
enzymes substrate. Supports used for ionic binding include
ion exchangers such as DEAE-cellulose. (b) Cross-linking with
bifunctional reagents to form insoluble aggregates. Reagents
used include GLUTARALDEHYDE (which binds enzymes via their
amino groups), or diamines (e.g. hexamethylenediamine) which
bind enzymes via their carboxyl groups after these groups have
been activated with carbodiimides; e.g., immobilized glucose
isomerase is manufactured by treating pellets of homogenized
cells of Bacillus coagulans with glutaraldehyde, yielding waterinsoluble aggregates containing glucose isomerase and other proteins. (c) Encapsulation. Enzymes are enclosed within LIPOSOMES
or hollow fibres which are permeable to low-MWt substrates
and products. (d) Entrapment within polymeric gels such as calcium ALGINATE, k-CARRAGEENAN and polyacrylamide. Enzymes
are added to a solution of the polymer which is then gelled e.g.
by the addition of a gelling agent. Leakage of enzymes from the
gel may be counteracted by cross-linking them e.g. with glutaraldehyde. Entrapment is suitable primarily for bioconversion
of low-MWt substrates which can diffuse through the gel.
Immobilized enzymes are used for simple one-step or twostep bioconversions in which there is no need for regeneration
of coenzymes. [Potential for immobilization of coenzymedependent enzymes: PTRSLB (1983) 300 335367.] In some
cases immobilization can improve the stability of enzymes which
may otherwise be inadequate under operational conditions; e.g.
immobilization of proteases inhibits their mutual degradation,
and multipoint binding of an enzyme to its support helps to
retain the conformational integrity of the enzyme protecting it
from inactivation by various denaturing agents (e.g. heat).
Immobilized cells can be used for bioconversions which are
not possible with isolated enzymes; the use of cells saves the cost
387
immune haemolysis
immunodeficiency The inability to respond with a normal
immune response to antigenic stimulation. (See also e.g. AIDS.)
immunodepression Syn. IMMUNOSUPPRESSION.
immunodiffusion See GEL DIFFUSION.
immunodominant See DETERMINANT and ANTIGENIC COMPETITION.
immunoelectron microscopy A procedure used e.g. for locating
particular antigens in cells or tissues. Essentially, the given
antigen is isolated and an antiserum is raised against it. The
homologous antibodies are labelled with e.g. FERRITIN and then
allowed to combine with the antigen in the cells or tissue; on
examination by transmission ELECTRON MICROSCOPY the location
of the given antigen is indicated by the ferritin label. (The use of
ferritin in this way is called the immunoferritin technique.) (cf.
IMMUNOSORBENT ELECTRON MICROSCOPY; see also IMMUNOGOLD
TECHNIQUE.)
immunoelectrophoresis (IEP) Any procedure in which antibodies (or other serum proteins) and/or antigens are subjected
to ELECTROPHORESIS prior to their detection, characterization,
or quantification (e.g. by means of specific antigenantibody
precipitation or staining). In one form of IEP the serum (or
other) sample is first subjected to electrophoresis in a strip of
agarose (or other) gel. This separates components into discrete
zones each zone containing one or more proteins characterized
by a specific electrophoretic mobility. (Some proteins migrate
in an unexpected direction see ELECTROENDOSMOSIS.) A rectangular slot (trough), cut into the gel strip parallel to the line
of electrophoretic migration, is filled with antiserum containing antibodies to some or all of the proteins in the sample; the
proteins and their homologous (and/or cross-reacting) antibodies diffuse through the agar and form lines or arcs of precipitate
where they meet in OPTIMAL PROPORTIONS (see GEL DIFFUSION).
(See also CHARGE-SHIFT IMMUNOELECTROPHORESIS; COUNTERCURRENT IMMUNOELECTROPHORESIS; ROCKET IMMUNOELECTROPHORESIS; TWO-DIMENSIONAL ELECTROPHORESIS.)
immunoferritin technique See IMMUNOELECTRON MICROSCOPY.
immunofluorescence The use of a fluorescent antibody (i.e. antibody conjugated with a FLUOROCHROME such as FITC, FLUORESCEIN, or RHODAMINE isothiocyanate) for the detection and/or
quantification of a specific antigen (or antibody). In the simplest
(direct) immunofluorescence techniques, used to detect antigen,
the specimen (tissue section, smear etc) is exposed to the conjugate (i.e. dye-linked antibody) for an appropriate time, washed
free of conjugate, and examined by fluorescence MICROSCOPY;
antigens homologous to the fluorescent antibodies are readily
identified by regions of fluorescence in the specimen. In the
indirect immunofluorescence technique (e.g. the indirect fluorescent antibody test, IFAT) the presence of a given antigen can be
determined by first exposing the specimen to unstained antibodies (e.g. a serum containing antibodies homologous to the given
antigen); the specimen is then washed free of uncombined antibodies, exposed to fluorescent anti-Ig antibodies, washed, and
examined by fluorescence microscopy. Any antigenantibody
combination on the specimen can thus be detected by the presence of fluorescent antibodies (which bind to the unstained antibodies); if particular antigens are known to be present in the
specimen, the test can be used to detect homologous antibodies in the serum. Another type of indirect immunofluorescence
technique is referred to as the SANDWICH TECHNIQUE.
In all immunofluorescence techniques adequate controls are
necessary to preclude an interpretation based on the non-specific
localization of conjugate, and to take into account any primary
FLUORESCENCE.
immunoradiometric assay
immunoliposome See LIPOSOME.
immunological drift Syn. ANTIGENIC DRIFT.
immunological paralysis IMMUNOLOGICAL TOLERANCE particularly that induced by pneumococcal polysaccharides.
immunological surveillance Syn. IMMUNOSURVEILLANCE.
immunological tolerance Inability to respond normally to a
given antigen (by humoral and/or by cell-mediated mechanisms)
as a consequence of prior exposure to that antigen; unrelated
antigens may elicit normal responses in the same individual.
(cf. SELF TOLERANCE.) Tolerance may be total (i.e. no detectable
response to antigen) or may involve e.g. failure to produce certain class(es) of antibody or some type(s) of immune response.
Failure to react normally to some antigens may be beneficial in
that harmful HYPERSENSITIVITY reactions may be avoided.
The extent, duration, and type of acquired tolerance is
influenced e.g. by the size of dose of the inducing antigen (the
toleragen), the nature of the antigen, the route of administration,
and the state of immunological maturity of the individual when
tolerance is induced; the induction of tolerance is inhibited e.g.
by adjuvants and is favoured e.g. by ANTIGENIC COMPETITION and
by non-specific immunosuppression.
Typically, thymus-dependent antigens (e.g. proteins) can
induce tolerance when administered in doses higher than the
normal immunizing dose (high-zone tolerance) or lower than
the normal immunizing dose (low-zone tolerance); in high-zone
tolerance both specific B cell and T cell clones are unresponsive
(clonal deletion), while in low-zone tolerance only the helper
T cell clone is unresponsive. Thymus-independent antigens usually induce only high-zone tolerance. Direct access of antigens to
the gastrointestinal tract favours the induction of tolerance (see
also SULZBERGERCHASE PHENOMENON). In general, tolerance to
a given antigen is more readily induced in the fetus or neonate
than in the adult, and in a naive subject than in a primed one.
The duration of tolerance may be extended by repeated administration of antigen.
Diverse mechanisms of tolerance induction have been suggested (including e.g. enhancement of suppressor T cell activity),
and different types of tolerance may involve different mechanisms. Exposure of immature B lymphocytes to specific antigen
or to anti-Ig makes them subsequently unresponsive (i.e., unable
to secrete antibody) when exposed to specific antigen (clonal
abortion); this suggests a reason why tolerance can be induced
more easily in the fetus or neonate than in adults.
immunological unresponsiveness (1) Syn. IMMUNOLOGICAL TOLERANCE. (2) Inability, or reduced ability, to respond to antigens
in general, due e.g. to IMMUNOSUPPRESSION.
immunomagnetic separation See DYNABEADS.
immunomodulation Specific or generalized alteration of the
immune response (see IMMUNOSTIMULATION; IMMUNOSUPPRESSION; IMMUNOLOGICAL TOLERANCE).
immunopathogenesis The development of pathological effects
as a direct result of the immune response.
immunoperoxidase method Any method in which antibodyconjugated, or otherwise complexed, peroxidases (e.g. horseradish peroxidase) are used to locate specific antigens on cells
or tissues (see e.g. ABC IMMUNOPEROXIDASE METHOD and PAP
TECHNIQUE).
immunopotentiation (1) Syn. IMMUNOSTIMULATION. (2) Nonspecific immunostimulation.
immunoprecipitable Capable of being precipitated by homologous antibodies.
immunoradiometric assay A highly sensitive IMMUNOASSAY by
which specific antigens are quantified using radioactive antibodies which may be prepared as follows. Antigen is adsorbed
immunorecessive
to an inert carrier (e.g. cellulose) and exposed to purified
immunoglobulins obtained from an antiserum containing the
homologous antibody; uncombined antibodies are removed by
washing, and the combined antibodies are radiolabelled (e.g.
with 125 I). The radioactive antibodies are then eluted for use in
the assay. In one form of assay, excess radioactive antibody is
added to the sample containing antigen at an unknown concentration; the reaction mixture is then exposed to fresh, cellulosebound antigen which adsorbs the uncombined antibodies and
permits their separation from the reaction mixture. The amount
of combined antibody can then be measured by determining
the level of radioactivity remaining in the reaction mixture; this
allows the concentration of antigen in the sample to be determined from a previously prepared standard curve (radioactivity
versus antigen concentration). (cf. RADIOIMMUNOASSAY.)
immunorecessive See DETERMINANT.
immunosilent See DETERMINANT.
immunosorbent assay Any IMMUNOASSAY in which antigen or
antibody is immobilized by adsorption to a solid surface see
e.g. ELISA.
immunosorbent electron microscopy (ISEM) ELECTRON MICROSCOPY in which particulate antigens (e.g. specific viruses) are
detected or examined by first complexing them with homologous
antibodies; prior to antigenantibody interaction the antibodies
may be e.g. fixed to an electron microscope grid (Derricks
method, antibody-coated grid technique, A-CGT), adsorbed to
a PROTEIN A-coated grid (Shuklas method, protein A-coated
grid technique, PA-CGT), or adsorbed directly to the protein
A of cells of Staphylococcus aureus (protein A-coated bacteria
technique, PA-CBT). [Review: AVR (1984) 29 169194.] (cf.
IMMUNOELECTRON MICROSCOPY.)
immunostaining The staining of a specific antigen or structure
by any method in which the stain (or stain-generating system) is
complexed with specific antibody (e.g. ABC IMMUNOPEROXIDASE
METHOD).
immunostimulation Specific or non-specific potentiation of the
immune response e.g. by the administration of a VACCINE or
by the use of an ADJUVANT. (cf. IMMUNOPOTENTIATION.)
immunosuppression (immune suppression) Complete or partial
suppression of normal IMMUNE RESPONSES either in respect of
specific antigen(s) (see also IMMUNOLOGICAL TOLERANCE) or in
respect of all antigens (generalized suppression). Immunosuppression can be induced e.g. by ionizing radiation; specific
antimetabolites (e.g. the folic acid antagonist methotrexate); a
variety of antimitotic/antitumour agents (e.g. 6-mercaptopurine,
prednisone, CYCLOSPORIN A, cyclophosphamide, azathioprine);
antilymphocyte serum. Immunosuppression induced by radiation
or by drugs tends to be generalized.
immunosurveillance The continual monitoring of the tissues for
abnormal antigens (e.g. on tumour cells) by cells of the immune
system.
immunotoxin An antibodytoxin conjugate intended to destroy
specific target cells (e.g. tumour cells) which bear antigens
homologous to the antibody. [Anti-CD22 immunotoxin BL22,
which uses a fragment of EXOTOXIN A, in chemotherapy-resistant
HAIRY-CELL LEUKAEMIA: NEJM (2001) 345 241247.]
Imotest A form of TUBERCULIN TEST in which a disposable plastic
unit is used. The tuberculin is contained in a sealed plastic tube
which is first broken and then squeezed to inoculate the nine
points used to penetrate the skin.
IMP Inosine 5 -monophosphate: see Appendix V(a).
impactor See AIR.
impedimetry A technique in which microbial growth and activity
are measured in terms of changes in the electrical impedence
incompatibility
incompatibility (in plasmids) The inability of PLASMIDS to coexist, stably, within the same cell when they have similar or
identical systems for replication (see PLASMID) and/or PARTITION.
Two incompatible plasmids which occupy the same cell will
(in the absence of a selective pressure for both plasmids) tend
to segregate to different cells during cell division. The stable
intracellular co-existence of one plasmid with another requires
that each plasmid be able to control, independently of the
other, its own replication/partition such that it can establish and
maintain a stable COPY NUMBER; the inability of a given plasmid
to maintain a stable copy number in the presence of another
plasmid is the characteristic feature of incompatibility.
In many cases, incompatibility arises from the synthesis of
plasmid-encoded trans-acting elements involved in the negative
control of plasmid replication. Since plasmids with identical
replication systems form identical trans-acting elements, the
elements synthesized by one plasmid will affect the replication
of other plasmids (in the same cell) which have an identical
replication system. In this case, plasmid replication initially
occurs randomly e.g., two (incompatible) plasmids will each
have an equal chance of being replicated. Once replicated,
however, a plasmid of one type will be present at a higher copy
number and will then be more likely to be involved in subsequent
rounds of replication; this effect tends to be cumulative and to
give rise to progeny cells that contain only one type of plasmid
(homoplasmid segregants).
In plasmids which have similar but not identical replication
systems, incompatibility may result in the preferential exclusion
of one particular plasmid; for example, in a cell containing
certain derivatives of the COLE1 PLASMID and of plasmid pMB1,
the ColE1 derivative is rapidly excluded possibly owing to
differential sensitivity of the two plasmids to RNA I. (See also
DISLODGEMENT and ONE-WAY INCOMPATIBILITY.)
In a number of plasmids the negative control elements which
govern incompatibility are small RNA molecules: see e.g. RNA I
under COLE1 PLASMID, and CopA under R1 PLASMID. In the pT181
family of Staphylococcus aureus plasmids, too, replication is
regulated by negative control elements (countertranscripts see
ANTISENSE RNA); however, in the pT181 family of plasmids
incompatibility is not governed by such elements because the
negative control elements of different plasmids in this group are
not interchangeable. Among pT181 plasmids incompatibility is
due to the existence of a common (interchangeable) Rep protein
(an initiator protein which promotes replication by binding to
the origin) [MGG (1986) 204 341348].
Incompatibility and the classification of plasmids. The expression of incompatibility or compatibility between plasmids provides a useful criterion for classifying them. Thus, plasmids are
classified into so-called incompatibility groups (Inc groups) in
such a way that all the plasmids in a given Inc group express
mutual incompatibility. Inc groups exist e.g. for plasmids which
occur in enterobacteria, and separate Inc groups exist for plasmids which occur in other bacteria; some (promiscuous) plasmids can occur e.g. in both enterobacteria and Pseudomonas spp,
and some of these plasmids have been allocated to an Inc group
in both the enterobacterial and pseudomonad grouping schemes.
Enterobacterial Inc groups are designated by the prefix Inc
followed by a letter and, sometimes, by a Roman numeral or a
Greek letter e.g. IncFII, IncIa. The letter (e.g. F, I) indicates
the type of conjugation system specified by the TRANSFER
OPERON; thus, e.g. an IncF plasmid specifies a conjugative
system like that of the F PLASMID or of an F-like plasmid,
and encodes either F pili or F-like pili (see PILI). The Roman
incompatible
numeral or Greek letter indicates a particular type of plasmid
replication system; thus e.g. IncFI and IncFII plasmids have
different replication systems (i.e., they are compatible) though
they specify similar conjugation systems. Some examples of
enterobacterial Inc groups are given below.
IncFI includes the F PLASMID, the COLICIN PLASMID ColV-K94,
and the R PLASMID R386.
IncFII includes the R1 PLASMID, R6 and R100.
IncIa (sometimes written IncI1 or IncI1 ) includes ColIb-P9,
the delta plasmid (see DELTA), and R64.
IncIg includes R621a.
IncN includes N3, R46, and R269N-1.
IncX includes the R6K PLASMID.
Pseudomonas Inc groups are designated IncP-1 to IncP-13,
the numbers referring to each of the 13 different types of
replication system. The conjugation systems of Pseudomonas
plasmids are less well known than those of enterobacterial
plasmids, but the pili encoded by Pseudomonas plasmids have
been characterized. [Pili encoded by Pseudomonas plasmids:
JGM (1983) 129 25452556; Pseudomonas R plasmids: Book
ref. 198, pp. 265293.] Some of the Pseudomonas Inc groups
are given below.
IncP-2 includes the CAM PLASMID, the OCT PLASMID, and the R
plasmid pMG1.
IncP-6 includes the R plasmid Rms149.
IncP-7 includes Rms148.
IncP-8 includes plasmid FP2 (which encodes resistance to
mercury).
IncP-9 includes R2, the SAL PLASMID, and the TOL PLASMID.
IncP-10 includes R91.
IncP-11 includes RP8 and R151.
IncP-12 includes R716.
IncP-13 includes pMG25.
Shared enterobacterial and pseudomonad Inc groups. Some of
the shared groups are given below, the enterobacterial Inc group
being given first.
IncC ( IncP-3) includes R55.
IncP ( IncP-1) includes R68, R751, RK2, RP1 and RP4.
IncQ ( IncP-4) includes RSF1010. (A plasmid apparently
related to this group, pFM739, has been isolated from Neisseria
sicca [JGM (1986) 132 24912496].)
incompatible (non-compatible) (plant pathol.) Refers to an interaction between a plant and a microorganism (e.g. an avirulent
strain of a pathogen) which does not result in the development
of disease in the plant. (cf. COMPATIBLE.)
incomplete antibodies (1) Syn. BLOCKING ANTIBODIES (sense 1).
(2) FAB PORTIONS.
incomplete Freunds adjuvant See FREUNDS ADJUVANT.
IncP groups See INCOMPATIBILITY.
IncQ group See INCOMPATIBILITY.
incubation The maintenance of e.g. inoculated media or other
types of material at a particular ambient temperature over a
period of hours, days, weeks, or longer; the purpose of incubation is to provide conditions suitable for growth etc. Incubation
is commonly carried out within closed, thermally insulated, thermostatically controlled chambers (incubators) or within vessels
suspended in a WATER BATH; refrigerated incubators maintain the
lower range of temperatures. Specialized incubation permits control of humidity, light, radiation etc as well as temperature. (cf.
PHYTOTRON.)
Cultures or specimens are sometimes left outside the incubator, i.e., they are exposed to the (often variable) conditions within
the laboratory a procedure known as incubation at room temperature.
incubation period (med., vet.) The time interval between INFECTION (sense 1), or e.g. exposure to a TOXIN, and the appearance
of the first symptoms of disease. (cf. PREPATENT PERIOD.)
incubator See INCUBATION.
IncX group See INCOMPATIBILITY.
independent assortment (genetics) During e.g. MEIOSIS: the
chance distribution of unlinked genes (see LINKAGE) among
progeny cells. Thus, e.g., if the (diploid) parent cell contained the
unlinked allelic pairs A/a and Z/z, any one of the four possible
allele combinations (A and Z, A and z, a and Z, a and z ) may
occur, with equal probability, in a given (haploid) progeny cell.
indicator (pH) See PH INDICATOR.
indicator organism Any organism whose presence and/or numbers serve to indicate the condition or quality of a material
or environment. For example, in studies on faecal pollution in
rivers, counts of the faecal bacteria Escherichia coli and Enterococcus faecalis are often used to indicate the degree of sewage
pollution at given sites. The same organisms are also used for
testing the efficiency of disinfection in treated drinking water,
their presence in treated water supplies indicating a failure of
the treatment process or contamination by sewage effluent subsequent to treatment. These organisms are used as indicators
because they are common intestinal bacteria: their presence in
water signals the potential presence of enteric pathogens. Water
samples are not routinely tested for each of the (many) different
types of enteric pathogen because, even in sewage-contaminated
water, a given pathogen may occur only intermittently. Moreover, in sewage-contaminated water the indicator bacteria greatly
outnumber pathogens so that they permit detection of very low
levels of faecal pollution. Endospores of Clostridium perfringens, which remain viable for long periods of time, have been
used to indicate previous contamination. Bifidobacterium spp
may specifically indicate human faecal pollution [JAB (1983)
55 349357], while faecal pollution from human and animal
sources may be differentiated by differences in the antibiotic
resistance patterns of faecal streptococci [AEM (1996) 62
39974002].
Traditional tests for faecal indicator bacteria include the
MULTIPLE-TUBE METHOD (for E. coli ) and membrane FILTRATION
for FAECAL STREPTOCOCCI.
Indicator organisms are also monitored in the assessment of
food-handling conditions/hygiene [indicator organisms in meat:
J. Food Protect. (1984) 47 672677].
(See also SAPROBITY SYSTEM and lichens and pollution in the
entry LICHEN.)
indigoidine See ERWINIA (E. chrysanthemi ).
indinavir See ANTIRETROVIRAL AGENTS.
indirect agglutination Syn. PASSIVE AGGLUTINATION.
indirect fluorescent antibody test (IFAT) See indirect IMMUNOFLUORESCENCE.
indirect immunofluorescence See IMMUNOFLUORESCENCE.
individual quick blanch (IQB) In the preparation of certain
foods for CANNING: blanching by exposure of individual items
of food to steam for a short period of time.
indole 3-acetic acid See AUXINS.
indole test An IMVIC TEST used to determine the ability of an
organism to produce indole from tryptophan [see Appendix
IV(f)]. The organism is grown in PEPTONE WATER or TRYPTONE
WATER at 37 C. (N.B. The presence of carbohydrate (which
may repress TRYPTOPHANASE) or nitrite in the medium can give
infectious bronchitis
in a positive test (i.e. indole produced), becomes pink or red.
(b) Xylene (ca. 1 ml) is added to ca. 5 ml of e.g. a 48-hour
culture with vigorous shaking (to extract the indole). EHRLICHS
REAGENT (ca. 0.5 ml) is then allowed to run down the side of the
slanted tube and forms a layer beneath the (floating) xylene; in
a positive test a red colour develops in the reagent layer. (c) An
oxalic acid-impregnated paper strip is inserted between the tube
and stopper before incubation; during incubation (up to 7 days)
indole (volatile at 37 C) reacts with the test strip to give a pink
or red colour.
indophenol oxidase test See OXIDASE TEST.
indoxyl acetate (3-acetoxyindole) A reagent used in identification tests for e.g. species of Arcobacter and Campylobacter.
Growth (from a non-selective medium) is suspended in distilled
water, and a paper disc, impregnated with indoxyl acetate, is
added; on incubation at room temperature for 20 minutes, a blue
coloration indicates hydrolysis of indoxyl acetate.
inducer exclusion (catabolite inhibition) The inhibition by glucose (or certain other readily metabolizable, preferred substrates) of the uptake of certain substrates by bacteria; for
example, if the bacteria are growing in a medium containing
two substrates, one of the substrates is preferentially taken up
and metabolized, and this substrate prevents the uptake of the
other.
There are several mechanisms for inducer exclusion; for
exclusion of e.g. lactose in enterobacteria see CATABOLITE
REPRESSION. Uptake of other (structurally unrelated) non-PTS
sugars e.g. maltose, melibiose is inhibited in a similar way.
In other cases, inducer exclusion may be due to competition
between structurally related substrates for the same transport
system or for shared components of the PTS; for example, in
enterobacteria glucose can directly inhibit the uptake of galactose
via a transport system common to both sugars.
In certain Gram-positive bacteria (e.g. Streptococcus spp,
Lactobacillus casei), accumulated sugar phosphates are actually expelled from the cell when e.g. glucose is added (inducer
expulsion); this involves a two-step mechanism in which intracellular dephosphorylation of the sugar is followed by efflux of
the free sugar. In these organisms regulation of sugar accumulation has been associated with the CcpA system (see CATABOLITE
REPRESSION); phosphorylation of HPr at the Ser-46 site reduces
its ability to be phosphorylated at the (routine) His-15 site by
enzyme I, and this should reduce phosphate transfer to the PTS
permeases and (hence) inhibit the uptake of sugars.
inducer expulsion See INDUCER EXCLUSION.
inducer protein Syn. activator: see OPERON.
induction (1) (of enzymes, gene expression) See e.g. OPERON.
(2) (of bacteriophage) See LYSOGENY.
industrial alcohol (microbiological aspects) Large amounts of
ethanol are produced commercially by the microbial fermentation of carbohydrates; ethanol is used primarily as a fuel (e.g. in
GASOHOL), as a solvent, and as a feedstock in the chemical industry. Fermentation ethanol (= fuel ethanol) may be produced
by the ALCOHOLIC FERMENTATION of substrates such as MOLASSES
and STARCH hydrolysates by strains of the yeast Saccharomyces;
laboratory- and pilot-scale evaluations have been made of the
economics of ethanol production from materials as diverse as
cassava, Jerusalem artichoke, LIGNOCELLULOSE, sweet sorghum
and WHEY using various yeasts, certain bacteria, and mixtures
of organisms.
Since many organisms can utilize only mono- or disaccharides, polymers such as cellulose and starch must be subjected
to acid or enzyme-catalysed hydrolysis before they can be fermented; strains of e.g. Clostridium thermocellum (which form
influenza virus C
Infection generally occurs by inhalation of virus-containing
aerosols, virions being deposited onto alveolar membrane or
(larger droplets) onto mucous membrane lining the respiratory
tract; in the latter case, virions may bind to sialic acid residues
in mucoproteins (rather than to receptors on respiratory epithelium) but such (abortive) binding can be broken by the viral
neuraminidase.
Incubation period: typically 13 days. Infection may be
asymptomatic, or there may be a sudden onset with chills, fever,
headache, muscular aches, anorexia, malaise etc.; fever subsides
after 15 days, and respiratory symptoms (coryza, cough etc.)
then become prominent. Recovery is usually rapid, although
cough and malaise may persist for several weeks.
Viral infection damages ciliated epithelium in the trachea and
bronchi; loss of cilia predisposes to secondary bacterial infection
and development of e.g. bronchial pneumonia involving organisms such as Streptococcus pneumoniae and/or Haemophilus
influenzae. Secondary infections are particularly problematic e.g.
in the elderly, debilitated and immunocompromised; apart from
pneumonia, secondary infections may lead to complications such
as tracheo-bronchitis, sinusitis, otitis media etc. (One early report
indicated that, in mice, the severity of disease can be reduced
by ozone [AEM (1982) 44 723731].)
Chemotherapy. Drugs such as AMANTADINE and rimantadine may afford some protection against influenza virus type
A if administered before or soon after infection. (See also
ZANAMIVIR.)
Vaccines. The original, formalin-inactivated, whole-virus vaccines produce local and systemic side-effects. Split-product
(split-virus) vaccines, containing H and N components of the
virus (as opposed to entire virions), are tolerated better.
Various alternative approaches to vaccines have been tried.
For example, attempts have been made to prepare attenuated
live vaccines by using REASSORTANT VIRUSes containing e.g.
surface glycoproteins from a currently epidemic strain and
internal components from an attenuated strain. In some cases
the attenuated strain was a temperature-sensitive (cold-adapted)
virus, while in other cases it was a strain from another species
with low virulence for man [e.g. avian strains: Book ref. 86,
pp 395405]. Vaccines have been prepared from synthetic
oligopeptides that mimic glycoprotein epitopes [oligopeptide
vaccines: MS (1984) 1 5558] and with virosomes [Lancet
(1994) 344 160163].
Owing to the effects of antigenic variation, the components
of influenza vaccines must be regularly reviewed to ensure that,
when used, a given vaccine will generate protection relevant to
the existing strain(s) of virus.
[Efficacy of influenza vaccines: RMM (1996) 7 2330.]
influenza virus A See INFLUENZAVIRUS.
influenza virus B See INFLUENZAVIRUS.
influenza virus C A virus of the ORTHOMYXOVIRIDAE. It is physicochemically and morphologically similar to members of the
genus INFLUENZAVIRUS, but differs in containing only 7 RNA
segments (total MWt ca. 45 106 ) and in having only one
type of surface glycoprotein (HA) which has both haemagglutinating and receptor-destroying activities, but apparently no
neuraminidase activity. It has been shown that, contrary to previous assumptions, sialic acid may nevertheless be an essential
component of the host cell-surface receptor [Virol. (1985) 141
144147]. Influenza virus C primarily infects man, although it
has been isolated from pigs in China; it generally causes only
mild or subclinical disease of the upper respiratory tract. Antigenic drifting occurs slowly, but antigenic shift has not been
observed (cf. INFLUENZAVIRUS).
Influenzavirus
are apparently resistant to drying at room temperature, and
survive at low temperatures in water. The virions can be
preserved for long periods at 70 C.
Infection of host cells; replication. The virion binds, via the
HA protein, to specific cell surface receptors containing sialic
acid residues; it is then internalized in a vesicle (endocytosis).
Low pH within the vesicle promotes cleavage of the HA protein
(by a host protease), and this leads to fusion of the viral envelope
with the vesicles membrane; as a result, viral ribonucleoprotein
and transcriptase are released into the cytoplasm of the host cell.
(See also ENVELOPE.)
The infectivity of a virion is abolished if antibodies have
bound to the globular HA1 portion of the HA glycoprotein.
Transcription of the (negative-sense) viral RNA occurs in
the nucleus; it involves viral transcriptase but depends on
the priming activity of the hosts (a-AMANITIN-sensitive) RNA
polymerase II. (See also RIBAVIRIN.) Transcription gives rise to
ten molecules of mRNA (two from each of genome segments 7
and 8 each of which have two reading frames). Viral mRNAs
are polyadenylated in the nucleus.
Replication of the viral genome also occurs in the nucleus and
involves viral transcriptase and the hosts RNA polymerase II.
The progeny ribonucleoprotein structures are assembled in the
nucleus, but details of the mode of assembly are not available.
HA and NA proteins are synthesized on rough endoplasmic
reticulum and subsequently migrate to localized sites in the
plasma membrane.
The type B influenzaviruses (but apparently not type A
viruses) encode another glycoprotein, NB, whose reading frame
overlaps that of NA; NB does not occur in the virion. Other
non-structural (NS) proteins are produced in cells infected with
A- or B-type viruses; their role(s) are unknown.
Maturation of the virion occurs by budding through the cell
membrane at sites containing HA and NA.
Classification/nomenclature of influenzaviruses. Influenzaviruses are classified as subtypes on the basis of their HA
antigens (15 different subtypes) and NA antigens (9 different
subtypes). A given strain of virus is designated by a formula
which indicates the following data: (i) type (i.e. A, B or C); (ii)
the animal from which the strain was first isolated (omitted if
the host was human); (iii) the place where the strain was first
isolated; (iv) the strain number; (v) the year of isolation; and
(vi) the particular HA (= H) and NA (= N) antigens. Example:
A/duck/Ukraine/1/63(H3N8)
The pandemic of 1957 so-called Asian flu was caused by a
strain formerly referred to as strain A2 but now designated:
A/Singapore/1/57(H2N2)
The 1968 pandemic so-called Hong Kong flu was due to:
A/Hong Kong/1/68(H3N2)
It appears that these two strains of influenzavirus were circulating human strains which had acquired novel antigens through
genetic reassortment with avian strains (see REASSORTANT VIRUS).
The sudden acquisition of new antigens (antigenic shift see
below) meant that radically new strains of virus had appeared
in a human population which, immunologically, was completely
naive.
It was previously assumed that if a new subtype appears
then the old strain ceases to circulate. However, subtype H1N1,
which was active early in the 20th century, re-appeared in 1977
and was involved in the pandemic of so-called Russian flu.
396
Inonotus
The surface glycoproteins of influenzaviruses undergo ANTIby this means, the virus may avoid the hosts
immune response and give rise to new outbreaks of influenza.
New strains of virus are generally not inactivated by antibodies induced by a previous strain i.e. antibody-based protection
tends to be strain-specific.
Variation in surface antigens may involve ANTIGENIC DRIFT or
ANTIGENIC SHIFT.
Antigenic drift involves relatively small changes in the surface
antigens, and this is associated with the regular occurrence of
epidemic influenza.
Antigenic shift involves major (and abrupt) changes in the surface antigens, and it happens infrequently. It has been recorded
only in type A influenzaviruses; this apparently reflects the fact
that type A strains can infect animals as well as man, and that,
in mixed infections (involving viruses from different species),
segments of the genome may undergo reassortment resulting
in the formation of novel hybrid subtypes containing genome
segments from different co-infecting parent virions.
In recent times, human strains typically displayed H1, H2
or H3, and N1, N2 or N3 antigens. Many other types of H
and N antigens occur in animal strains, suggesting scope for the
formation of new pandemic strains by reassortment. Fortunately,
influenzaviruses are generally highly species-specific so that
transfer across the species barrier is assumed to occur only
rarely. Transfer occurred when American harbour seals were
infected by an avian H7N7 virus in 1980 [Virology (1981) 113
712724] and pigs were infected by avian strains [JV (1996) 70
80418046].
Transfer across the species barrier may occur in a two-step
process; for example, transmission of the human H3N2 subtype
to avian hosts can be achieved after reassortment in pigs.
The 1997 outbreak of bird flu in Hong Kong, which caused
six deaths, resulted from avian-to-human transmission of a fowl
plague strain (H5N1). Subsequently, no deaths from this strain
were reported following large-scale slaughter of poultry.
In 1999, two children in Hong Kong were infected with
influenza A subtype H9N2 (strains A/Hong Kong/1073/99;
A/Hong Kong/1074/99); these strains closely resemble a strain
isolated from quail in 1997 (A/quail/Hong Kong/G1/97). Also in
1999, H9N2 viruses were isolated from patients with influenzalike illness in Guangdong province (China).
The H5N1 and (Hong Kong) H9N2 human isolates are similar
in the six genes that encode internal components of the virion,
suggesting that H9N2 arose from reassortment of H5N1. Avian
strains with these six genes might have a tendency to infect
humans and may therefore have the potential to give rise to a
novel human pathogen. [Relationship between H9N2 and H5N1
human isolates: PNAS (2000) 97 96549658].
H5N1 caused over 50 human deaths in East Asia in
20042005. Isolates from humans and those from birds consisted of two distinct clades. In all isolates the genes were of
avian influenzaviruses, indicating that they were not derived
through reassortment with human strains. Human-to-human
transmission was described. [Evolution of H5N1 avian influenza
viruses in Asia: EID (2005) 11(10). Influenza (special issue):
EID (2006) 12(1) (January).]
informational suppressor See SUPPRESSOR MUTATION.
informosome See MRNA (b).
infraciliature (ciliate protozool.) The subpellicular system which
includes the kinetosomes and all the various associated microfibrillar and microtubular structures (see e.g. KINETODESMA; POSTCILIARY MICROTUBULES; TRANSVERSE MICROTUBULES).
GENIC VARIATION;
397
inoperculate
RFI v strand at a specific site in the IG region; the free 3 end is
elongated as in other ssDNA phages (q.v.). Genome lengths of
displaced v ssDNA are cleaved by gp2, and each is circularized
to form v ss cccDNA. At first, new v strands are converted
to RFs. However, a phage-coded SSB protein (gp5) gradually
accumulates, eventually coating the newly formed v strands and
blocking their conversion to RFs (stage III). Phage coat proteins
(at least gp8 and gp3) are synthesized as soluble cytoplasmic
precursors with a signal peptide at the amino end (see SIGNAL
HYPOTHESIS); these proteins become inserted asymmetrically into
the cytoplasmic membrane, the signal peptides are removed, and
the proteins are anchored within the membrane [PNAS (1982)
79 52005204]. Phage assembly which requires THIOREDOXIN
[PNAS (1985) 82 2933] occurs (in f1) at zones of adhesion
between the cytoplasmic and outer membranes, f1 gp1 possibly
being involved in the formation of these adhesion zones [JB
(1985) 163 12701274] (cf. ADHESION SITE); gp8 displaces gp5,
and the mature virion is finally extruded through the host cell
envelope.
insect diseases Bacterial pathogens of insects include e.g. Bacillus spp (see e.g. AMERICAN FOULBROOD, DELTA-ENDOTOXIN, MILKY
DISEASE), Melissococcus pluton (see EUROPEAN FOULBROOD), and
species of RICKETTSIELLA, SERRATIA and SPIROPLASMA. (See also
CECROPINS and SARCOTOXINS.)
Fungal entomopathogens include species of e.g. Ascosphaera
(see CHALK-BROOD); ASCHERSONIA; Aspergillus (see e.g. STONEBROOD); BEAUVERIA; Coelomomyces (see BLASTOCLADIALES);
CORDYCEPS; CULICINOMYCES; ENTOMOPHTHORA, ERYNIA and other
fungi of the ENTOMOPHTHORALES; FUSARIUM; HIRSUTELLA; METARHIZIUM; NOMURAEA; SEPTOBASIDIALES; TERMITARIA; VERTICILLIUM.
Protozoal entomopathogens include e.g. species of MALPIGHAMOEBA, NOSEMA and THELOHANIA. (See also CRITHIDIA,
HERPETOMONAS and LEPTOMONAS.)
For viral entomopathogens see e.g. BACULOVIRIDAE; CYTOPLASMIC POLYHEDROSIS VIRUS GROUP; DENSOVIRUS; DROSOPHILA X
VIRUS; ENTOMOPOXVIRINAE; FLACHERIE; HOUSEFLY VIRUS; NODAVIRIDAE; NUDAURELIA b VIRUS GROUP; PICORNAVIRIDAE; POLYDNAVIRIDAE; SIGMA VIRUS.
(See also INVERTEBRATE DISEASES and BIOLOGICAL CONTROL.)
insect iridescent viruses See CHLORIRIDOVIRUS and IRIDOVIRUS.
insectmicrobe associations See e.g. AMBROSIA FUNGI; DUTCH
ELM DISEASE; FUNGUS GARDENS; FUNGUS GNATS; INSECT DISEASES; MYCETOCYTE; TERMITEMICROBE ASSOCIATIONS; WOODWASP FUNGI.
insecticidal crystal protein (ICP) See BIOLOGICAL CONTROL.
insertion mutation (addition mutation) A type of MUTATION in
which one or more nucleotides are inserted into the genome;
if the number of nucleotides inserted is not divisible by
3, the mutation will be a FRAMESHIFT MUTATION. Insertion
mutations commonly result from the insertion of a TRANSPOSABLE
ELEMENT or prophage (see also BACTERIOPHAGE CONVERSION). (cf.
DELETION MUTATION.)
insertion sequence (IS element) A TRANSPOSABLE ELEMENT
which contains no genetic information other than that necessary
for its transposition. (cf. TRANSPOSON.) An IS element may
transpose independently, when it may be detectable by the
effect(s) of its insertion at a new site, or it may occur as a
terminal part of a composite (class I) TRANSPOSON. An IS element
is defined by its ends: an INVERTED REPEAT sequence of ca. 1040
bp has been found to occur at both ends in every IS element
so far analysed; these inverted repeats are apparently necessary
for transposition and are probably the recognition sites for the
intein
integrative suppression The phenomenon in which the integration of a plasmid into a bacterial chromosome suppresses the
effect of a chromosomal mutation which has inhibited the initiation of chromosome replication; replication of the joint plasmidchromosome replicon is apparently initiated at a site within
the plasmid. Thus, e.g., as a result of integrative suppression, a
temperature-sensitive dnaA mutant of Escherichia coli can carry
out limited chromosome replication at a non-permissive temperature.
integrins A family of CELL ADHESION MOLECULES found on various types of cell and involved in many aspects of cell physiology; the molecule is a heterodimer of proteins consisting of
an a subunit non-covalently linked to a b subunit the particular combination of a subunit (many types) and b subunit (few
types) determining the biological activity of each integrin.
Integrins of the b1 subfamily are found e.g. on various
types of epithelial cell either on the basolateral surface or
(e.g. a6 b1 ) on the basal surface (i.e. adjacent to the basement
membrane) [integrins (review): HJ (1993) 25 469477]. These
integrins have a major role in cellcell and cellmatrix interaction binding to ligands that include collagen, fibronectin and
laminin; however, such interaction involves more than cell position and maintenance of tissue structure: integrinligand binding
can also trigger signals that modulate a wide range of cell functions, including aspects of the cell cycle.
The b1 integrins are also implicated as receptors for the
adhesins of invasive pathogenic bacteria; for example, adhesins
of Yersinia enterocolitica have been found to bind (in vitro) to
the a5 b1 integrin of epithelial cells.
The b2 integrins are found primarily on leukocytes; their
expression on a given cell is apparently dependent on activation e.g. cytokine-stimulated cells may exhibit the leukocyte function-associated antigen-1 (LFA-1; = CD11a/CD18; =
aL b2 ) and the Mac-1 integrin (= CD11b/CD18; = aM b2 ); both
of these integrins can bind to ICAM ligands (see IMMUNOGLOBULIN SUPERFAMILY and INFLAMMATION).
The b2 integrins can also serve as receptors for bacterial
adhesins. Thus, many integrins bind (via their a subunit)
to ligands that contain the amino acid sequence Arg-GlyAsp (RGD), and this sequence is mimicked by the adhesin
filamentous haemagglutinin (FHA) of Bordetella pertussis; the
binding between FHA (RGD sequence) and Mac-1 (aM b2 ) of an
activated macrophage assists bacterial invasion of the phagocyte.
The b3 integrin aIIb b3 (gpIIbIIIa; = CD41b/CD61) is found
on platelets and megakaryocytes; its ligands include fibrinogen,
VON WILLEBRAND FACTOR and fibronectin. Failure to synthesize
adequate amounts of this integrin results in deficient platelet
aggregation (Glanzmanns thrombasthenia).
(See also LEUKOCYTE ADHESION DEFICIENCY.)
[Defects in human integrins: Lancet (1999) 353 341343.]
integron A region of DNA which includes (i) a gene encoding a
site-specific recombinase (see SITE-SPECIFIC RECOMBINATION) and
(ii) a corresponding site for recombination into which one or
more genes may be inserted [see e.g. JAC (1999) 43 14].
Integrons may have a role as a general gene-capture mechanism
in bacterial evolution [PNAS (2001) 98 652657].
intein In certain types of protein: an internal sequence of amino
acids apparently capable of catalysing a self-splicing reaction
in which the intein is excised (forming a separate protein)
and the terminal parts of the original polypeptide (the two
exteins) are joined to form a functional protein. [Review: TIBS
(1995) 20 351356. Intein sequences (review): NAR (1997) 25
10871093.]
interallelic complementation
interallelic complementation See COMPLEMENTATION TEST.
intercalary Not apical or terminal: e.g. formed or situated
between apex and base of a given structure or between two
cells in a chain of cells.
intercalating agent Any dye possessing a planar chromophore
which can insert (intercalate) between adjacent base pairs in
dsDNA or in base-paired regions in ssDNA (e.g. HAIRPIN
loops); bifunctional (bis) intercalating agents have two such
chromophores per molecule (see e.g. QUINOXALINE ANTIBIOTICS).
Intercalation forces the base pairs apart and causes (a) local
unwinding of the helix, the degree of unwinding (unwinding
angle, f) depending on the nature of the dye, and (b) an increase
in the length of the DNA. In linear dsDNA these effects lead
to an increase in viscosity and a decrease in sedimentation
coefficient (s) of the DNA in proportion to the amount of dye
intercalated. Intercalative binding is limited to a maximum of
one dye molecule per 23 bp; the binding of a dye molecule
at one site precludes binding of others at the adjacent sites (the
neighbour exclusion principle).
In circular dsDNA intercalation causes a local increase in
pitch and thus a decrease in local (and hence average overall)
twist. It follows from W r = Lk T w (see DNA) that, as
increasing amounts of dye intercalate in a negatively supercoiled
molecule, the amount of writhe progressively decreases to
zero (molecule behaves as relaxed), and then increases again
as the molecule becomes positively supercoiled. The changes
in writhe are accompanied by changes in viscosity of the
DNA solution (increase to a maximum, then decrease) and in
sedimentation coefficient of the DNA (decrease, then increase).
Since intercalation relieves the strain of negative supercoiling,
a negatively supercoiled cccDNA molecule has a higher affinity
for intercalating agents than does the equivalent nicked or linear
DNA, while a relaxed or positively supercoiled cccDNA has
a lower affinity than the equivalent nicked or linear DNA.
However, a cccDNA molecule has a limited capacity to unwind,
and can therefore bind fewer molecules of intercalating agent
than can equivalent linear or nicked circular DNA molecules
(see e.g. ETHIDIUM BROMIDE).
Many intercalating agents have antimicrobial and antitumour
activity, inhibiting e.g. transcription, DNA replication etc, and
inducing FRAMESHIFT MUTATIONS. In vivo, intercalation is often
followed by DNA strand breakage, possibly due to the action
of nucleases which recognize distortion of the helix at the
intercalation sites. At lower concentrations some intercalators
(e.g. aminoACRIDINES, ETHIDIUM BROMIDE) can cause the selective
loss of small cccDNAs such as plasmids (see CURING (2)),
mtDNA (see PETITE MUTANT), ctDNA, and kinetoplast DNA. (See
also ACTINOMYCIN D; ANTHRACYCLINE ANTIBIOTICS; QUINOXALINE
ANTIBIOTICS; TILORONE. cf. MITOMYCIN C and PSORALENS.)
[Review of DNA-binding drugs: Bioch. J. (1987) 243 113.]
intercistronic complementation See COMPLEMENTATION TEST.
intercrines Syn. CHEMOKINES; thus, a-intercrines = a-chemokines, b-intercrines = b-chemokines.
interesterification An industrial process in which fatty acyl
residues are interchanged among the various triglycerides in a
mixture of lipids; the process, which is catalysed e.g. by sodium
methoxide, is carried out in order to modify the composition
(and hence properties) of oils and fats. Interesterification can be
carried out using certain microbial LIPASES for the production of
useful mixtures of triglycerides which cannot be made by conventional chemical processes. [Enzyme-catalysed modification
of oils and fats: PTRSLB (1985) 310 227233.]
interference (1) (virol.) The phenomenon in which the replication of one virus (the challenge virus) is partially or completely
interleukin-1
an enzyme, RNase L (also called RNase F), which can cleave
viral and cellular RNA; however, 25A is unstable, being
enzymically degraded by 2 ,5 -phosphodiesterase.
The antiviral activity of interferons has been assayed in vitro
by a plaque-reduction method in which cultured cells are treated
with IFN and subsequently challenged with virus; the titre of
IFN may be taken as the reciprocal of the highest dilution of
IFN that produces a 50% decrease in the number of plaques.
Therapeutic uses of interferons. Both natural and recombinant forms of interferon (types I and II) have been evaluated for clinical use in a range of diseases, including various
types of malignancy, Kaposis sarcoma (IFN-a), multiple sclerosis (IFN-b), diseases of viral aetiology, and disease caused
by Mycobacterium tuberculosis (IFN-g). Commercial products
include Alferon N (multicomponent IFN-a; Interferon Sciences,
USA); Betaferon and Betaseron (recombinant IFN-b; Schering
AG); Gammaferon (recombinant IFN-g; Rentschler, Germany).
[Clinical uses of interferons: Book ref. 226, pp 237271.]
The enhanced capacity of lymphocytes to secrete IFN-g
when thalidomide is used for adjuvant therapy may offer an
explanation for the ability of thalidomide to bring about clinical
improvement in patients infected with e.g. Mycobacterium
tuberculosis and HIV [AAC (2000) 44 22862290].
(See also ELISPOT ASSAY (for TB).)
intergenic complementation See COMPLEMENTATION TEST.
intergenic repeat unit Syn. ERIC SEQUENCE.
intergenic spacer region See RIBOTYPING.
intergenic suppression See SUPPRESSOR MUTATION.
intergenote A partial zygote formed by heterologous TRANSFORMATION (i.e., transformation in which the donor DNA is derived
from a species different from that of the recipient).
intergranal frets See CHLOROPLAST.
interkinesis See MEIOSIS.
interkinetal Refers e.g. to the plane of cell division typical of
members of the OPALINATA: longitudinal, between the rows of
kineties. (cf. HOMOTHETOGENIC.)
interleukin-1 (IL-1) A cytokine (see INTERLEUKINS) secreted by
various types of cell, including monocytes, fibroblasts, dendritic
cells and endothelial cells. There are several forms of IL-1: IL1a (previously called lymphocyte activating factor, LAF) and
IL-1b (both pro-inflammatory cytokines with similar or identical
functions) and IL-1ra; IL-1ra binds to the cognate receptor of
IL-1a and IL-1b but, having no agonist activity, it functions
as an antagonist of the a and b forms of IL-1. (There are two
types of receptor for IL-1 but only one is functional; the other
(decoy) receptor does not initiate intracellular signals when
IL-1a or IL-1b binds to it.)
For IL-1g see INTERLEUKIN-18.
The mature forms of IL-1a and IL-1b are produced by
intracellular cleavage of precursor pro-proteins. IL-1b is cleaved
(activated) by a cysteine protease referred to as IL-1b-converting
enzyme (ICE). (ICE also has a role in APOPTOSIS.)
Cells stimulated to produce IL-1 generally form both the a
and b types; however, in at least some cases (e.g. a monocyte
responding to LPS), the amount of IL-b produced is much
greater than that of IL-1a.
The known or presumed functions of IL-1a and IL-1b in vivo
include:
Activation, and induction of cytokine synthesis in macrophages.
Induction of ACUTE-PHASE PROTEINS in the liver.
Stimulation of activated B cells to proliferate and form
antibody (and possibly stimulation of T cells).
401
interleukin-2
but, unlike e.g. TNF, it does not induce shock when administered
experimentally.
interleukin-10 (IL-10) A cytokine (see INTERLEUKINS) produced
e.g. by the Th2 subset of T cells and by monocytes stimulated
by LPS. IL-10 has anti-inflammatory activity; for example,
it inhibits proliferation and release of cytokines in antigenstimulated Th1 cells, it inhibits release of pro-inflammatory
cytokines from monocytes and macrophages, and it promotes
proliferation and synthesis of antibodies in activated B cells.
interleukin-12 (IL-12; natural killer stimulatory factor) A cytokine (see INTERLEUKINS) produced by B cells and also by
macrophages acting as antigen-presenting cells. IL-12 appears to
be essential for development of the Th1 subset of T cells from
naive T cells; it also stimulates cytotoxicity in NK cells and
enhances the release of cytokines from NK cells, macrophages
and T cells. IL-12 also has anti-angiogenic activity (it inhibits
development of new blood vessels).
The ability of macrophages to synthesize IL-12 is inhibited by
the binding of measles virus to the complement receptor CD46.
interleukin-18 (syn. interleukin-1g) An INTERLEUKIN produced
e.g. by macrophages, keratinocytes and (murine) Kupffer cells.
IL-18 is a pro-inflammatory cytokine which induces IFN-g in
T cells (and murine spleen cells), enhances cytotoxicity in NK
cells, and promotes the Th1 (rather than Th2) immune response.
IL-18 also triggers activation of NF-kB and synthesis of e.g.
IL-1b, TNF-a and Fas ligand.
IL-18 is synthesized in a biologically inactive form; it is
activated by IL-1b converting enzyme (ICE; also referred to
as caspase-1).
IL-18-mediated induction of IFN-g can be inhibited by the
binding of poxvirus-encoded proteins to IL-18 [PNAS (1999)
96 1153711542 (correction: PNAS (2000) 97 11673)].
interleukin-21 An INTERLEUKIN which, in vitro, influences the
proliferation/maturation of NK cells from bone marrow, the
proliferation of B cells co-stimulated with anti-CD40, and the
proliferation of T cells co-stimulated with anti-CD3. IL-21 is
synthesized by activated CD4+ T cells. [Nature (2000) 408
5763.]
interleukins Certain CYTOKINES which are secreted by, and
effective on, leukocytes (white blood cells) but which, in
some cases, can also be secreted by other types of cell (e.g.
endothelial cells). It should be noted that the nomenclature
is inconsistent in that some cytokines which conform to this
description (e.g. tumour necrosis factor) are not formally referred
to as interleukins; moreover, some interleukins are also classified
in other named categories (e.g. interleukin-8 is a chemokine).
Each interleukin (IL) is designated by a number e.g. IL-4,
IL-6, IL-21.
(See also separate entries for individual interleukins.)
intermediate filaments (IFs; IMFs) In most types of eukaryotic
cell: protein filaments, ca. 711 nm thick, which form part of the
CYTOSKELETON. IMFs appear to be much more stable than either
microfilaments or microtubules, and their roles are believed to
include the strengthening of the cytoskeleton. IMFs differ e.g.
according to cell type and species, and the monomers of different
IMFs vary widely in size; the monomer vimentin (MWt ca.
55000) occurs in many types of cell.
intermediate host In heteroxenous coccidia: the host in which
the asexual phase occurs (see EIMERIORINA).
internal guide sequence See SPLIT GENE (b).
internalin A See LISTERIOSIS.
interphase (1) See MITOSIS. (2) See DICTYOSTELIOMYCETES.
interrupted gene Syn. SPLIT GENE.
Induction of synthesis of endothelial adhesion molecules during INFLAMMATION; induction of e.g. IL-1 and colony-stimulating
factors in endothelial cells.
Induction of fever (apparently by stimulation of prostaglandins
in the temperature regulatory region of the brain).
The biological activities of IL-1 overlap with those of tumour
necrosis factor (TNF); IL-1b and TNF-a have been found to be
synergistic when jointly administered to animals. Moreover, IL1b and TNF-a stimulate the production of each other (as well as
their own synthesis). However, despite the overlap in activities,
it appears that, unlike TNF-a, IL-1 cannot promote cytotoxic
activity via apoptosis.
interleukin-2 (IL-2; killer helper factor, KHF; T cell growth
factor, TCGF) A cytokine (see INTERLEUKINS) produced by
T lymphocytes. In vitro, IL-2 can stimulate proliferation of
antigenically or mitogenically activated T cells; in vivo, it
appears to promote the growth/differentiation of T cells and to
enhance the cytotoxicity of CD8+ T cells and NK cells. (See
also CD28 and ANTIBODY FORMATION.)
IL-2 promotes development of the Th1 subset of T lymphocytes, and is one of the cytokines secreted by these proinflammatory cells.
The gene encoding IL-2 (like that encoding IFN-g) contains
three introns.
(See also SEVERE COMBINED IMMUNODEFICIENCY.)
interleukin-4 (IL-4) A cytokine (see INTERLEUKINS) produced by
lymphocytes of the Th2 subset. IL-4 promotes differentiation
of Th0 to Th2 cells, and in antigenically stimulated B cells it
seems to e.g. induce class switching to IgG4 and IgE (IgG1
and IgE in mice). IL-4 is also involved in the formation of
eosinophils probably through its ability to promote the Th2
subset and (consequent) secretion of interleukin-5 (a cytokine
required for the normal development of eosinophils).
The ability of naive CD4+ T cells to secrete IL-4 is inhibited
when ICAM-1 is co-expressed with antigen on the antigenpresenting cell [PNAS (1999) 96 30233028].
interleukin-5 (IL-5) A cytokine (see INTERLEUKINS) produced by
the Th2 subset of T lymphocytes (see also INTERLEUKIN-4). IL5 appears to be the main stimulus for eosinophilia in certain
parasitic infections. [Eosinophilia and helminthic infections:
BCH (2000) 13 301317.]
interleukin-6 (IL-6) A cytokine (see INTERLEUKINS) produced by
a variety of cells, including monocytes/macrophages, fibroblasts,
endothelial cells and the Th2 subset of T lymphocytes. Synthesis
of IL-6 in monocytes/macrophages can be induced by LPS
(lipopolysaccharides) or by cytokines (TNF-a or IL-1); the P
FIMBRIAE of uropathogenic Escherichia coli are reported to be
potent inducers of IL-6.
IL-6 appears to have many roles in vivo. These roles include
stimulation of growth, differentiation and antibody production
in B cells, and induction of ACUTE-PHASE PROTEINS; in at least
some cases IL-6 may contribute to the development of fever.
interleukin-8 (IL-8) A cytokine (see INTERLEUKINS) produced
by many types of cell, including monocytes/macrophages,
neutrophils, fibroblasts, epithelial and endothelial cells, keratinocytes, NK cells and T cells. Agents that stimulate production of IL-8 include LPS and the cytokines IL-1 and TNF;
production of IL-8 is inhibited by certain cytokines (e.g. IFN-g
and IL-4) and by glucocorticoids.
IL-8 acts as a chemoattractant and activator primarily for
neutrophils (see CHEMOKINES), and its main role in vivo is
believed to be the recruitment of leukocytes to sites of infection/INFLAMMATION. IL-8 is found in many inflammatory diseases
402
invertase
intravital staining See VITAL STAINING.
intrinsic resistance (to antibiotics) See ANTIBIOTIC.
intron See SPLIT GENE.
intron homing (in bacteria) The process in which introns (of
either group I or group II) spread, in replicative fashion, to allelic
intron-less genes. The mechanism of intron homing differs in the
two types of intron.
Intron homing in group I introns is initiated when a DNA
endonuclease (homing endonuclease), encoded within the intron
sequence, acts at the potential insertion site in an intron-less
allele, typically making a double-stranded cut. The lesion is
repaired by enzymes which use the intron-containing gene as
a template; in this way, a copy of the intron is synthesized in
the insertion site of the intron-less allele.
In group II introns, the process begins with an intron-encoded
protein which forms a complex with an RNA copy of the intron.
This RNAprotein (RNP) complex is able to recognize the
insertion site in an intron-less allele. The RNP complex can
then (i) cut both strands at the target site, covalently inserting the
RNA into one strand, and (ii) form a cDNA copy of the RNA
(by virtue of the proteins reverse transcriptase function); the
RNA is then replaced by DNA. The involvement of a reversetranscribed copy of the intron (cf. group I introns) is reflected
in the term retrohoming for the process in bacterial group II
introns. Intron homing (in both group I and II bacterial introns)
is outlined in a recent minireview [JB (2000) 182 52815289
(52815282)].
inulin A linear FRUCTAN consisting of (2 1)-b-linked fructofuranose residues. Inulins occur e.g. as storage polysaccharides
in certain plants (e.g. in dahlia tubers).
inulinase An enzyme (b-fructosidase, 2,1-b-D-fructan-fructanohydrolase, EC 3.2.1.7) which hydrolyses INULIN to FRUCTOSE.
Many microbial inulinases also show INVERTASE activity, and
some can hydrolyse bacterial LEVAN. Microbial inulinases may
prove useful in the commercial production of fructose from plant
inulins [AAM (1983) 29 139176].
inv gene (Yersinia) See FOOD POISONING (Yersinia).
invspa genes See PATHOGENICITY ISLAND and FOOD POISONING
(Salmonella).
invasin In certain pathogenic bacteria: a type of cell-surface
molecule which promotes uptake of the pathogen by (eukaryotic)
host cells. Examples of invasins include invasin (see FOOD
POISONING (Yersinia)) and internalin A (see LISTERIOSIS). In
strains of UPEC (q.v.), the FimH adhesin appears to function
as an invasin.
invasion (of phagocytes by pathogens) See end of section (a) in
PHAGOCYTOSIS.
invasiveness (of a pathogenic microorganism) The ability of a
pathogen to spread through a hosts tissues; the degree of
invasiveness reflects the relative insusceptibility of the pathogen
to the hosts defense mechanisms. (See also AGGRESSIN.)
invasomes See FOOD POISONING (Salmonella).
inversion (mol. biol.) See e.g. CHROMOSOME ABERRATION and
RECOMBINATIONAL REGULATION.
invert sugar See INVERTASE.
invertase (1) (saccharase; sucrase; b-fructosidase; b-D-fructofuranoside fructohydrolase; EC 3.2.1.26) An enzyme which
hydrolyses SUCROSE to glucose and fructose; it can also hydrolyse
raffinose to fructose and melibiose. Invertase occurs in many
yeasts and other fungi and in higher plants; it is obtained
commercially mainly from BAKERS YEAST in which it occurs
in the cell wall as a mannoprotein containing ca. 50% mannose.
Invertase is used chiefly in the conversion of sucrose to invert
invertebrate diseases
molecular form (I2 ); however, an iodine solution was reported to
inactivate poliovirus (at 25 C) more efficiently at pH 10 than at
pH 6 (at pH 10 iodine occurs mainly as hypoiodous acid, HIO)
[AEM (1982) 44 10641071]. Both I2 and HIO are strongly
microbicidal; the ratio I2 :HIO in a solution of iodine is affected
not only by pH but also by the total concentration of dissolved
iodine and by the presence of organic matter [Book ref. 65,
pp. 183196]. The staining, corrosive and irritant properties of
iodine can be overcome by complexing the element with certain
high-MWt surface-active compounds e.g. polyvinyl pyrrolidone, certain quaternary ammonium compounds; such complexes are referred to as iodophores (or iodophors). Iodophores
have the antimicrobial properties of iodine together with the
detergent properties of the surfactant, but only ca. 80% of the
bound iodine is released; their response to pH is similar to that
of iodine. Iodophores have been used e.g. for the disinfection of
swimming-pool water and dairy equipment; polyvinyl pyrrolidoneiodine (povidoneiodine, PVPiodine) has been used for
treating skin and mucous membrane infections involving species
of Streptococcus, Staphylococcus and Candida. Betadine and
Wescodyne are iodophores used as antiseptics/disinfectants. (cf.
IODOFORM; IODONIUM COMPOUNDS; see also CHLORINE.)
(b) (as a stain) See e.g. LUGOLS IODINE.
iodinin A red, water-soluble pigment: 1,6-phenazinediol-5,10dioxide; crystals of iodinin are formed in the culture medium
e.g. by Microbispora parva.
iodochlorohydroxyquin See 8-HYDROXYQUINOLINE.
5-iodo-2 -deoxyuridine Syn. IDOXURIDINE.
iodoform (CHI3 ) A compound once widely used as an antiseptic;
its antimicrobial activity is poor compared with that of IODINE.
iodonium compounds Compounds of the form R2 IX, in which R
is an organic group and X is an inorganic ion; such compounds
(e.g. diphenyliodonium chloride) contain trivalent iodine, are
strongly basic, and possess antimicrobial properties, but their
activity against spores is doubtful.
iodophores (iodophors) See IODINE (a).
ion-exchange chromatography See CHROMATOGRAPHY.
ion-motive force phosphorylation See ELECTRON TRANSPORT
PHOSPHORYLATION.
ion transport Ion fluxes across ENERGY-TRANSDUCING MEMBRANES are involved e.g. in certain types of energy conversion
(see e.g. PROTON ATPASE, PROTON PPASE, END-PRODUCT EFFLUX),
in the ion-linked uptake of certain substrates, in the regulation
of intracellular osmotic pressure and pH, in the generation of
electrochemical gradients of specific ions, and (apparently) in
morphogenetic processes (see GROWTH (fungal)). Since ions cannot pass freely across such membranes (cf. OUTER MEMBRANE)
their transmembrane translocation requires a driving force and
more or less specific TRANSPORT SYSTEMS which may involve
UNIPORT, ANTIPORT or SYMPORT processes. The energy needed
for transmembrane ion translocation may be provided, directly,
by (a) a concentration gradient of the ion itself; (b) a gradient of another ion e.g. H+ (see pmf in CHEMIOSMOSIS) or Na+
(see SODIUM MOTIVE FORCE); (c) ATP hydrolysis (see e.g. PROTON
ATPASE); (d) the direct coupling of metabolism to ion transport
(see ELECTRON TRANSPORT CHAIN and SODIUM MOTIVE FORCE); or
(e) light (see PHOTOSYNTHESIS and PURPLE MEMBRANE).
Ion electrochemical gradients as driving forces in ion transport. A difference in the concentrations of a given ion on
either side of a membrane constitutes an electrochemical gradient
which may be able to provide a driving force for the transmembrane transfer of the ion itself or of other types of ion. However,
the presence of such a gradient, and the existence of transmembrane route(s) for a given ion, does not necessarily mean that
ionizing radiation
the ion will be translocated: ion transport is subject to various
intracellular and extracellular regulatory factors; moreover, the
transmembrane route taken by a given ion may vary according
e.g. to the extracellular concentration of that ion.
The potential energy of a transmembrane gradient of ions
can be considered in terms of the change in Gibbs free energy
which occurs when a charged species is transferred down an
electrochemical gradient. Thus, e.g., if one mole of an ion,
Xm+ , is transferred down an electrical potential gradient of 1y
millivolts, from concentration [Xm+ ] to [Xm+ ] , the net change
in Gibbs free energy (1G) can be obtained from the general
electrochemical equation:
1G = mF1y + 2.3RT log10
[Xm+ ]
[Xm+ ]
(1)
[Xm+ ]
[Xm+ ]
(2)
[Xm+ ]int
Z
log10 m+
m
[X ]ext
(3)
b-ionone ring
genome of two linear pieces of dsRNA (MWts ca. 2.3 106
and 2.5 106 ). Each strand of both RNA molecules is covalently linked by its 5 end to a protein the first known case
of genome-linked protein in a dsRNA virus. A minor protein
component (VP105) is reputed to have dsRNA-dependent RNA
transcriptase activity. [Review: CJM (1983) 29 377384.] Virus
transmission occurs vertically and horizontally.
IPNV is representative of a family of bisegmented dsRNA
animal viruses, Birnaviridae [approved: Intervirol. (1986) 25
141143], which includes the INFECTIOUS BURSAL DISEASE VIRUS
of chickens, DROSOPHILA X VIRUS, and various IPNV-like
viruses isolated from freshwater and marine fish (e.g. Eel Virus
European, EVE, isolated from Japanese eels: Anguilla japonica;
see also SPINNING DISEASE) and from marine bivalve molluscs
(e.g. oysters Ostrea and Crassostrea spp and Tellina tenuis).
ipomeamarone The (+)-enantiomer of 2-methyl-2-(4-methyl-2oxopentyl)-5-(3-furyl) tetrahydrofuran: a PHYTOALEXIN produced
by the sweet potato (Ipomoea batatas) in response to infection by certain fungal pathogens (e.g. the black rot fungus
Ceratocystis fimbriata). Ipomeamarone and its ()-enantiomer
ngaione (a normal constituent of certain trees and shrubs) are
both hepatotoxic and can cause liver disease in livestock. (See
also 4-IPOMEANOL.)
4-ipomeanol A substance, (1-(3-furyl)-4-hydroxy-1-pentanone),
produced by the sweet potato (Ipomoea batatas) in response to
infection by certain fungal pathogens. It is toxic to animals, causing pulmonary oedema and massive pleural effusion. Together
with e.g. ipomeanine (a dihydro derivative of 4-ipomeanol) it
may be the lung oedema factor responsible for the fatal respiratory disease in livestock (especially cattle) which follows ingestion of mould-damaged sweet potatoes. (cf. IPOMEAMARONE.)
iprodione See DICARBOXIMIDES.
IPTG Isopropyl-b-D-thiogalactoside: a gratuitous inducer of the
LAC OPERON.
IQB INDIVIDUAL QUICK BLANCH.
IR INVERTED REPEAT.
Ir genes Immune response genes: genes, associated with the
MHC, which determine the ability of a mouse to make humoral
and cell-mediated immune responses to a wide range of antigens;
certain of these genes encode the IA ANTIGENS.
Irgasan DP 33 Syn. TRICLOSAN.
Iridaea See RHODOPHYTA.
iridescence Coloured light formed by interference when white
light is reflected from both surfaces of a thin film.
iridescent insect viruses See CHLORIRIDOVIRUS and IRIDOVIRUS.
Iridia See FORAMINIFERIDA.
Iridoviridae A family of icosahedral dsDNA-containing VIRUSes
which infect invertebrates (mainly insects) and poikilothermic
vertebrates. The family contains four genera: CHLORIRIDOVIRUS,
IRIDOVIRUS, LYMPHOCYSTIVIRUS and RANAVIRUS. (cf. AFRICAN
SWINE FEVER.)
Virion: icosahedral (ca. 120300 nm diam.) and complex in
structure, consisting of a nucleoprotein core surrounded by a
layer composed of a lipoprotein membrane beneath an icosahedral protein lattice. Some virions may have an additional
lipoprotein ENVELOPE derived from the host cell plasmalemma or
endoplasmic reticulum; the envelope is apparently not essential
for infectivity. Virions are generally stable at pH 310 and at
4 C; they can be inactivated e.g. at 55 C for 1530 min. Members of the genera Ranavirus and Lymphocystivirus are sensitive
to ether and non-ionic detergents.
Genome: one molecule (possibly two in some cases) of linear
dsDNA (MWt ca. 100250 106 ); in at least some iridoviruses
Ionizing radiations sterilize by supplying energy which permits a great variety of lethal chemical reactions to occur
in contaminating organisms. In general, resistance to ionizing radiation increases in the order: multicellular organisms;
Gram-negative bacteria; Gram-positive bacteria and moulds;
bacterial endospores, viruses and viroids. Exceptions include e.g.
Deinococcus radiodurans, which is more resistant than most or
all bacterial endospores. Low (sublethal) doses of radiation can
be mutagenic: e.g., in Escherichia coli the SOS SYSTEM and
hence error-prone (mutagenic) repair may be induced. (In
some cases, susceptibility to ionizing radiation is enhanced by
the presence of water and/or oxygen.) Typically, toxins and
other microbial products are more resistant than cells to ionizing
radiations. Ionizing radiation may affect the materials being sterilized e.g., a sterilizing dose of radiation can damage certain
plastics.
Large-scale industrial sterilization is generally carried out with
either a source of gamma-rays or a source of high-energy electrons. In a gamma-radiation plant the source of radiation is 60 Co
(cobalt-60): a radioactive isotope (half-life ca. 5.3 years) which
provides both gamma-rays and (relatively) low-energy electrons.
High-energy electrons (ca. 510 MeV) are produced in electron
accelerators. The high-energy electron radiation used for sterilization carries more energy than does the gamma-radiation,
although it has poorer powers of penetration; sterilization processes using high-energy electrons require exposures of the order
of seconds, while those using gamma-rays require minutes or
hours. The actual sterilizing dose used should, ideally, take into
account e.g. the numbers and types of contaminants. In many
countries the recommended minimum sterilizing dose is ca. 2.5
Mrad (25 kGy, see GRAY); a higher minimum is recommended
in Scandinavia.
X-rays (a form of electromagnetic radiation) have been used
e.g. for sterilizing items of high density which are impermeable
to a beam of high-energy electrons.
[Quality assurance in radiation sterilization (theoretical treatment): JAB (1985) 58 303313.]
(See also ULTRAVIOLET RADIATION.)
b-ionone ring See CAROTENOIDS.
ionophore Any substance which actually or effectively increases
the permeability of biological membranes (or of artificial
lipid bilayers) to one or more types of ion. Channel-forming
ionophores (e.g. GRAMICIDINS) form pores in the membrane; such
ionophores typically exhibit little discrimination between different ions, and may allow the passage of up to ca. 107 ions per pore
per second. Mobile carrier ionophores (e.g. PROTON TRANSLOCATORS) diffuse within the membrane; they can exhibit a high
degree of specificity for ions. Mobile carriers may effect ion UNIPORT (see e.g. VALINOMYCIN) or ion ANTIPORT (see e.g. A23187 and
NIGERICIN). (See also ENNIATINS, LASALOCID, MACROTETRALIDES,
SALINOMYCIN and ION TRANSPORT.)
Iotech process A process, involving explosive depressurization,
in which the ligninhemicellulosecellulose complex from plant
material is disrupted to release CELLULOSE for use as a feedstock
in certain biotechnological processes (e.g. SINGLE-CELL PROTEIN
or INDUSTRIAL ALCOHOL production).
IP10 (chemokine) See CHEMOKINES.
IpaA protein See DYSENTERY.
IpaB protein See APOPTOSIS, DYSENTERY and PROTEIN SECRETION
(type III systems).
IPN virus (IPNV) The causal agent of INFECTIOUS PANCREATIC
NECROSIS disease of salmonid fish. The virion has an unenveloped, icosahedral capsid (ca. 59 nm diam.) containing a
406
ironsulphur proteins
Listeria monocytogenes uses siderophores from other bacteria
and various iron-chelating agents in the environment and mammalian hosts; a cell-surface ferric reductase may recognize all
of these agents.
A pathogens absolute need for iron has prompted the search
for new vaccines that stimulate protective antibodies against the
cell-surface receptors for iron-chelating agents.
Pseudomonas aeruginosa can reduce PYOCYANIN to leucopyocyanin which, in turn, can reduce the (ferric) iron in iron
transferrin complexes [Inf. Immun. (1986) 52 263270]; iron
thus released from transferrin may be available to iron-limited
bacteria.
Virulence in the fish pathogen Vibrio anguillarum (see VIBRIO)
depends partly on a plasmid-encoded siderophore, anguibactin.
[Plasmid-mediated iron transport and bacterial virulence: ARM
(1984) 38 6989.]
In plant-pathogenic Erwinia chrysanthemi, mutants defective
in iron transport were non-pathogenic [JB (1985) 163 221227].
[Iron metabolism in pathogenic bacteria: ARM (2000) 54
881941.]
Applied aspects. Siderophore-producing strains of Pseudomonas putida used for the BACTERIZATION of seed potatoes apparently increase the yield in short-rotation crops [NJPP (1986) 92
249256]; thus, siderophores may modify the RHIZOSPHERE microflora in favour of the potato plant. Interestingly, some microbial
ferrisiderophores are taken up by plants [see for example FEBS
(1986) 209 147151].
iron bacteria Bacteria whose growth is associated with the extracellular deposition of oxides or hydroxides of iron and/or manganese; such deposits usually cover or impregnate the bacterial
capsule, sheath or stalk. Iron bacteria occur e.g. in various ironand manganese-containing soils and waters, and in water distribution systems (see also TUBERCLE (sense 2)). Evidence that
the deposition of metal oxides/hydroxides is a direct result of
microbial metabolism has not been obtained for the majority
of the iron bacteria (cf. GALLIONELLA) many of which have
not even been grown in pure culture; the opportunity for biological oxidation of Fe2+ is relatively poor under aerobic conditions (in which Fe2+ undergoes rapid autoxidation) but becomes
significant under microaerobic conditions, particularly at pH
56, in which autoxidation is slow. (Autoxidation of Mn2+ is
slow below pH 9.) The iron bacteria include e.g. CLONOTHRIX,
CRENOTHRIX, GALLIONELLA, LEPTOTHRIX, METALLOGENIUM, OCHROBIUM and SIDEROCAPSA; some authors include the acidophilic iron
oxidizers, e.g. Thiobacillus ferrooxidans.
[Review: ARM (1984) 38 515550.]
iron box See OPERATOR.
iron corrosion See CATHODIC DEPOLARIZATION THEORY.
ironsulphur centre See IRONSULPHUR PROTEINS.
ironsulphur proteins (FeS proteins) A category of iron- and
sulphur-containing proteins which are widely distributed in cells
of all types and which participate e.g. in electron transfer processes (see e.g. ELECTRON TRANSPORT CHAIN and NITROGENASE);
except in rubredoxins (see later) each ironsulphur protein contains two or more iron atoms linked to one another by an equal
number of (acid-labile) sulphur atoms, the entire complement
of iron and acid-labile sulphur forming one or more discrete
ironsulphur centres (= ironsulphur clusters) linked to the
protein typically by thiolate side-chains of cysteine residues.
(See also RHODANESE.)
Rubredoxins are traditionally included with the FeS proteins, although they contain only one iron atom and no acidlabile sulphur; the iron is linked to the protein via four thiolate
ironophores
ligands. A rubredoxin with an Em of ca. 60 mV occurs in
Clostridium pasteurianum. (See also HYDROCARBONS.)
Other ironsulphur proteins contain, per molecule, one or
more of the following types of centre: [2Fe2S] (see also RIESKE
PROTEIN), [3Fe3S] (found e.g. in Azotobacter vinelandii ),
and/or [4Fe4S]; 2S, 3S and 4S refer specifically to acid-labile
sulphur.
Ironsulphur proteins can be classified as either simple (e.g.
rubredoxins, FERREDOXINS) or complex (= conjugated), the latter
having additional prosthetic groups such as a flavin or haem or a
non-iron metal atom (e.g. molybdenum). Complex ironsulphur
proteins include e.g. the sulphite reductase of Escherichia coli
(EC 1.8.7.1), which includes four [4Fe4S] centres together
with molecules of FAD, FMN and sirohaem, and a chloroplast
nitrate reductase (EC 1.7.7.1) containing one [4Fe4S] centre
and sirohaem.
[Review: Book ref. 146, pp. 79120.]
ironophores Syn. SIDEROPHORES.
Irpex See APHYLLOPHORALES (Polyporaceae).
IRS Internal resolution site: see Tn3.
IS element See INSERTION SEQUENCE.
IS1 A 768-bp INSERTION SEQUENCE present e.g. in R plasmids (see
also Tn9 ), the genome of BACTERIOPHAGE P1, the chromosome
of Escherichia coli K12 (in multiple copies), etc. IS1 seems to
transpose preferentially to target sites which are rich in AT, frequently cleaving at a GC pair within such a region. Transposition
can apparently generate either 9- or 8-bp duplications of target
DNA [PNAS (1985) 82 839843]. IS1 encodes two genes, insA
and insB, which are required for IS1-mediated transposition and
cointegration.
IS5 A 1195-bp INSERTION SEQUENCE present in the chromosome
of Escherichia coli K12 strains; it has a high target specificity
(see TRANSPOSABLE ELEMENT).
IS10 An INSERTION SEQUENCE that has been found only in association with Tn10 (q.v.).
IS50 See Tn5.
IS101 A 209-bp INSERTION SEQUENCE which is defective and
carries no genes; its transposition depends entirely on gdencoded transposase and resolvase functions (see Tn3 ). (cf.
Tn951.) Its inverted repeat sequences are closely related to, but
not identical with, those of gd.
IS900 An INSERTION SEQUENCE reported to be specific to Mycobacterium paratuberculosis. IS900 has been used e.g. as a target
for PCR-based detection of M. paratuberculosis in milk [AEM
(1998) 64 31533158].
IS1000 Syn. gd (see Tn3 ).
IS6110 An INSERTION SEQUENCE regarded as specific to members
of the Mycobacterium tuberculosis complex (i.e. M. tuberculosis,
M. bovis, BCG, M. africanum and M. microti ). The number of
copies of IS6110 per genome varies with strain; a few strains of
M. tuberculosis apparently lack the sequence, while most strains
of M. bovis appear to contain only a single copy. Some 16 copies
of IS6110 occur in the genome of the H37rv reference strain of
M. tuberculosis [Nature (1998) 393 537544].
Some authors have questioned the specificity of IS6110,
indicating that a central region of the sequence is similar to
a sequence in non-tuberculous mycobacteria [JCM (1997) 35
799800]; others have affirmed the specificity of this sequence
for members of the M. tuberculosis complex [JCM (1997) 35
800801].
IS6110 has been widely used for TYPING isolates of
M. tuberculosis. However, using SPOLIGOTYPING, some authors
have found that, in a particular subset of multidrug-resistant
itraconazole
isopsoralen See PCR.
isopycnic centrifugation See CENTRIFUGATION.
isorenieratene See LIGHT-HARVESTING COMPLEX.
isoschizomers RESTRICTION ENDONUCLEASES which recognize the
same sequence in DNA but which are derived from different
species. [Restriction endonucleases and their isoschizomers:
NAR (1991) 19 20772109.]
Isosphaera See BACTERIA (taxonomy).
Isospora A genus of parasitic protozoa (suborder EIMERIORINA)
which form disporic, tetrazoic oocysts (cf. e.g. EIMERIA); the
genus, as originally defined, includes only homoxenous species,
but it has been expanded by some authors [see AP (1982)
20 403406] to include heteroxenous species which form
disporic, tetrazoic oocysts (typically shed unsporulated) and
which may form tissue cysts in the intermediate host. The
expanded genus thus includes e.g. organisms otherwise placed in
the genera BESNOITIA and TOXOPLASMA, as well as the obligately
heteroxenous Isospora datusi (= Hammondia hammondi).
For generalized homoxenous and heteroxenous life cycles see
EIMERIORINA; see also COCCIDIOSIS (q.v. for refs).
Isosticha See HYPOTRICHIDA.
isosulfazecin See MONOBACTAMS.
isotopic labelling (probe) See PROBE.
Isotricha A genus of ciliates related to DASYTRICHA.
isotype (class) Each of the five main variant forms (classes) of
IMMUNOGLOBULIN (IgA, IgD, IgE, IgG and IgM); isotypes differ
in the amino acid sequence in the constant region of their heavy
chains. Immunoglobulins of all five isotypes occur in every
normal individual (cf. ALLOTYPE).
A given isotype may be divided into subclasses (distinguishable serologically). For example, there are several subclasses of
IgG (designated IgG1, IgG2 etc.).
isotype switching See ANTIBODY FORMATION.
isovelleral See LACTARIUS.
IsoVitaleX A commercial preparation containing e.g. vitamin
B12 , amino acids, purines, D-glucose, thiamine and TPP, NAD+ ,
Fe(NO3 )3 , PABA used for the enrichment of media for
isolating and/or cultivating fastidious bacteria (e.g. Haemophilus
spp).
isozyme Syn. ISOENZYME.
Issatchenkia A genus of yeasts (family SACCHAROMYCETACEAE)
which reproduce by multilateral budding; pseudomycelium is
formed. Asci are persistent. Ascospores: spheroidal, roughsurfaced. Cells contain ubiquinone-7 (Q-7). Sugars may be
fermented; NO3 is not assimilated. A pellicle develops on
liquid cultures. Species I. occidentalis (anamorph: Candida
sorbosa), I. orientalis (anamorph: Candida krusei ), I. scutulata,
I. terricola have been isolated from soil, fruit, etc. [Book
ref. 100, pp. 214223.]
isthmus (biol.) Any narrow region connecting two structures in
an organism or cell: see e.g. placoderm DESMIDS.
iteron One of a number of repeated (reiterated) nucleotide
sequences which occur in and/or near the replication origin(s)
in certain plasmids e.g. the F PLASMID and the R6K PLASMID.
Itersonilia
A genus of fungi incertae sedis; the organisms
form mycelium containing CLAMP CONNECTIONS, and it has
been suggested that I. perplexans forms a one-spored basidium
[TBMS (1983) 80 365368].
itraconazole A clinically useful AZOLE ANTIFUNGAL AGENT (a
triazole); it has a high MWt and is highly lipophilic. Itraconazole
has a broad spectrum of activity, inhibiting yeasts, dimorphic
fungi and filamentous fungi; it appears to be less toxic to
mammalian tissues than e.g. miconazole or ketoconazole owing
IUB
IVET (in vivo expression technology) A technique used for
detecting those genes (of a pathogen) which are transcribed only
during infection of the host; such genes may be virulence genes,
and this can be studied further e.g. by animal tests involving
strains of the pathogen which are mutant for the given gene.
IVET is outlined in the figure.
[Some examples of IVET: TIM (1997) 5 509513. Behaviour
of bacteria in the host, and the methodology for studying it: TIM
(1998) 6 239243.]
IVS (mol. biol.) Intervening sequence (= intron): see SPLIT GENE.
iwatake The edible lichen Umbilicaria esculenta.
to its much higher selectivity for the fungal rather than the
mammalian cytochrome P-450. [Review: Arch. Derm. (1986)
122 399402.]
[Pharmocology of itraconazole (review): Drugs (2001) 61
(supplement 1) 2737.]
IUB International Union of Biochemistry.
iucAiucD genes See SIDEROPHORES.
IUdR See IDOXURIDINE.
IUPAC International Union of Pure and Applied Chemistry.
iutA gene See SIDEROPHORES.
ivanolysin See THIOL-ACTIVATED CYTOLYSINS.
IVET (in vivo expression technology): the principle (diagrammatic). The figure shows one of several forms of IVET.
IVET detects those genes of a pathogen whose expression is induced during (and only during) infection of the host animal.
Vector molecules (see top, right) are inserted, by transformation, into a population of cells of the pathogen. In each transformed cell, the
(random) fragment of chromosome in the vector inserts into the corresponding part of the pathogens chromosome (by an insertionduplication
mechanism); because the vector molecules contain different fragments of the chromosome they will insert into different chromosomal sites in
different cells forming a heterogeneous population of recombinant cells.
In some recombinant cells, the vectors two promoter-less genes will have been inserted in frame with an upstream promoter. In such
cells, both of these genes will be transcribed if the promoter is active.
The recombinant cells of the pathogen are used to infect a test animal whose food contains the antibiotic chloramphenicol (to which the
pathogen is normally susceptible). Under these conditions, a recombinant cell can grow only if it produces chloramphenicol acetyltransferase
(CAT), i.e. only if the CAT gene (in the vector molecule) is controlled by an active promoter; thus, the fact that a given recombinant cell grows
within the animal indicates that its CAT gene is controlled by a promoter which is active within the test animal. (Because synthesis of CAT
points to an active promoter, the CAT gene is sometimes called a reporter gene.) Cells producing CAT can form large populations which
greatly outnumber cells that do not form CAT.
We need to know whether the promoter controlling an expressed CAT gene is active only when the pathogen is in the test animal or
whether it is also active when the pathogen is cultured (e.g. on agar media). If active only in the test animal, this indicates that the gene
normally controlled by that promoter is induced during infection; such a gene is of interest because of its possible association with virulence.
To study promoter activity further, the recovered bacteria are plated on a medium which lacks chloramphenicol but which contains the agent
XGAL (q.v.); all the cells will grow. If a given promoter is active in culture then b-galactosidase will be formed and will give rise to a blue-green
colony; such a colony tells us that activation of the given promoter does not occur only within the test animal. A white (lac ) colony indicates
that b-galactosidase (and CAT) can be formed only within the test animal, i.e. the relevant promoter is active only when the pathogen is actually
infecting the animal. The gene which is normally controlled by this promoter can be isolated, cloned and sequenced and examined for its role
in virulence.
Reproduced from Bacteria, 5th edition, Figure 11.3, pages 304305, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN
0471-98880-4) with permission from the publisher.
410
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
J
J chain A cystine-rich polypeptide (MWt ca. 15000) involved in
the formation of dimeric and polymeric forms of both IgA and
IgM (q.v.). In an IgA dimer the J chain forms a link between
cystine residues situated near the C-terminal ends of the heavy
chains in the two monomers.
jaagsiekte (pulmonary adenomatosis) A SHEEP DISEASE characterized by chronic progressive pneumonia in which the alveolar spaces become occluded by adenomatous ingrowths of the
epithelium; the causal agent(s) appear to be viral (a herpesvirus
and/or a retrovirus), but the causal agent of MAEDI is not
involved. Incubation period: 13 years. Symptoms: dyspnoea,
emaciation, and a profuse watery nasal discharge which may
contain hyperplastic adenomatous epithelial cells; fever and
inflammation are absent. Death occurs within ca. 4 months.
[Book ref. 33, pp. 807808.]
Jaccard coefficient See entry SJ .
jack bean lectin CONCANAVALIN A.
jack-in-the-box ascus Syn. BITUNICATE ASCUS.
Jacquard coefficient See entry SJ .
JAK See CYTOKINES.
janiemycin A polypeptide ANTIBIOTIC which inhibits transglycosylation in PEPTIDOGLYCAN synthesis.
Janthinobacterium
A genus of Gram-negative, strictly aerobic, catalase-positive, chemoorganotrophic bacteria which occur
e.g. in soil and water; the organisms are motile (flagellated)
rods, 0.81.2 2.56.0 m. Metabolism is respiratory (oxidative); acid (no gas) is formed from e.g. glucose. Growth occurs
in/on simple media (e.g. peptone water); violet, often gelatinous,
colonies are formed on nutrient agar. Optimum growth temperature: 25 C, maximum 32 C. MR ve; VP ve; usually oxidase
+ve. GC%: ca. 6167. Type species: J. lividum (formerly Chromobacterium lividum). [Book ref. 22, pp. 376377.]
Janus green A blue basic DYE which has both azine and azo
chromophores; it is used e.g. in VITAL STAINING.
Janus kinase See CYTOKINES.
Japanese B encephalitis (Japanese encephalitis; Russian autumn
encephalitis) A viral ENCEPHALITIS which affects man, pigs and
horses; it occurs in epidemics in e.g. Japan, China, Korea and
parts of India. The disease is usually acute, but may run a
protracted course with acute exacerbations. The causal agent is a
flavivirus (see FLAVIVIRIDAE) which occurs e.g. in wild birds and
is transmitted by mosquitoes (usually Culex sp). An inactivated
vaccine has been used in Japan. [Review: ARM (1986) 40
395414.]
Japanese river fever Syn. SCRUB TYPHUS.
Japonochytrium See THRAUSTOCHYTRIDS.
JarischHerxheimer reaction (Herxheimer reaction) A potentially fatal reaction which may follow the first effective
chemotherapy against e.g. brucellosis or syphilis or, in general,
diseases caused by certain bacteria (particularly spirochaetes)
and protozoa. Symptoms (e.g. an initial rise in temperature) are
associated with a cascade of CYTOKINES which seem to be responsible for at least some of the pathophysiology. [Review: BCID
(1994) 1 6574.] The reaction has been prevented by treatment
with antibodies against tumour necrosis factor (TNF) [NEJM
(1996) 335 311315].
jarrah dieback A disease of the jarrah (Eucalyptus marginata)
an important timber tree e.g. in Western Australia; the causal
agent is generally believed to be Phytophthora cinnamomi, but
JonesMote sensitivity
by hydrogen bonding as e.g. in early intermediates formed
during homologous RECOMBINATION.
JonesMote sensitivity (cutaneous basophil hypersensitivity) A
form of hypersensitivity which may develop e.g. when a human
subject is primed with a soluble protein antigen, or a guinea
pig is primed with a protein in incomplete Freunds adjuvant;
subsequent challenge with the relevant allergen (within a few
days of priming) leads to a weak, non-indurated, erythematous
skin reaction in which the lesion contains a high proportion of
BASOPHILS. (These reponses do not occur in mice.) JonesMote
sensitivity can be transferred to a non-primed animal by serum
(cf. DELAYED HYPERSENSITIVITY).
Jonesia
A genus which contains the former species Listeria
denitrificans [IJSB (1987) 37 266270].
Jopling reactions See LEPROSY.
JPC See JUNCTIONAL PORE COMPLEX.
Jud. Comm. JUDICIAL COMMISSION.
Judicial Commission A taxonomic body concerned with the
interpretation and/or amendment of the rules of microbial
nomenclature.
412
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
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K
and antitumour activity. In the presence of divalent cations,
kanchanomycin binds to DNA and inhibits DNA and RNA
synthesis.
Kaposis sarcoma (KS) A rare multifocal neoplastic disease
which occurs in two forms: (i) slow and indolent (limited mainly
to the skin), and (ii) rapid and fulminant (involving skin and
gastrointestinal tract). The milder form occurs in certain ethnic
groups (e.g. Ashkenazi Jews). The aggressive form occurs in
children in tropical Africa and is also a common feature in HIVinfected patients. (Note that Kaposis sarcoma occurs also in
some immunosuppressed transplant patients.)
Kaposis sarcoma appears to be associated with human
(gamma) herpesvirus 8 (HHV8) [see e.g. Lancet (1997) 349
558563] in conjunction with the immunosuppressive effects of
HIV. [PCR-based investigation of HHV8 in KS biopsies: Am. J.
Path. (1997) 150 147153.] Activation of latent HHV8 in vitro
has been achieved by demethylation of the promoter of a transactivator region by means of the reagent tetradecanoylphorbol
acetate (TPA), and studies on the level of methylation of the
transactivator region in biopsies have suggested a relationship
between methylation status and the development of HHV8associated disease [PNAS (2001) 98 41194124].
Kaposis varicelliform eruption May refer either to eczema
herpeticum or eczema vaccinatum (see ECZEMA).
kappa chain See LIGHT CHAIN.
kappa particles See CAEDIBACTER.
Karatomorpha See PROTEROMONADIDA.
Karber method See END-POINT DILUTION ASSAY.
Karelian fever See SINDBIS VIRUS.
Karnal bunt (partial bunt; new bunt) A wheat disease caused
by Neovossia indica (formerly e.g. Tilletia indica); originally a minor disease confined to NW India, it has recently
spread through northern India and has become established in
Afghanistan, Iraq, Pakistan, and Mexico, apparently transmitted
on and in wheat seed. Usually only some of the grains in an
ear are attacked; infected parts of the grain are initially grey
but gradually turn black and emit a foul odour (trimethylamine).
[Bot. Rev. (1983) 49 309330.] (See also COMMON BUNT.)
karyogamy The coalescence of nuclei (cf. PLASMOGAMY).
karyogram See KARYOTYPE.
karyokinesis Syn. MITOSIS.
karyological relict (ciliate protozool.) Any present-day ciliate
whose characteristics (particularly nuclear constitution) resemble
those of (presumably) phylogenetically ancient ciliates. (See also
KARYORELICTID GYMNOSTOMES and PRIMOCILIATID GYMNOSTOMES.)
karyolysis (histopathol.) The dissolution of a cells nucleus with
consequent loss of affinity for basic dyes. (cf. KARYORRHEXIS.)
karyomastigont A nucleus together with its associated flagellum
(or flagella) and, when present, axostyle. (See also DIPLOMONADIDA.)
karyomere See MACRONUCLEUS.
karyonide (caryonide) (ciliate protozool.) A clone of cells in
which all the macronuclei have been derived from the same
macronucleus.
karyoplast A nucleus which has been isolated from a (eukaryotic) cell and which is enclosed within a sac of cytoplasmic
membrane containing a small amount of cytoplasm. (cf. CYTOPLAST.)
karyorelictid gymnostomes
Kawasaki disease An acute, occasionally fatal, febrile disease of unknown cause which affects infants and young
children. Kawasaki disease may be a manifestation of an
immune-complex-mediated systemic vasculitis [ADC (1984) 59
405409]; more recently it has been suggested that at least some
of the symptoms may be due to a SUPERANTIGEN.
kb (kilobase) Of a DNA or RNA strand: a unit of length equal to
103 bases; the unit may also be used for 103 base pairs (bp) in
dsDNA or dsRNA although kbp (kilobase-pairs) is also used
in this context.
kbp See previous entry.
Kcat mechanism See PHASEOLOTOXIN.
KCN broth (cyanide broth; Mllers [= Moellers] cyanide
medium; potassium cyanide broth) A MEDIUM used in the
CYANIDE TEST; it consists of an aqueous solution of peptone
(1.0%), NaCl (0.5%), KH2 PO4 (0.0225%), Na2 HPO4 (0.56%),
and KCN (0.0075%). The medium may be stored at 4 C for up
to ca. 2 weeks.
KCN test See CYANIDE TEST.
kDa Kilodalton: 103 DALTONS.
kDNA KINETOPLAST DNA.
KDO See LIPOPOLYSACCHARIDE.
Kdp system See ION TRANSPORT.
kefir A fermented milk beverage made in parts of Russia, Bulgaria and the former Yugoslavia. Milk is fermented by a mixed
and varied population of organisms which usually include lactobacilli [SAAM (1983) 4 286294; JAB (1984) 56 503505],
Lactococcus lactis, and yeasts (for example, Saccharomyces
spp); lactic acid, ethanol and carbon dioxide (which causes foaming) are the main products. The organisms become embedded in
an extracellular polysaccharide (kefiran) to form whitish, gelatinous granules [scanning electron microscopy: JAB (1980) 48
265268] which are carried to the surface by bubbles of carbon
dioxide. The granules are collected and used as an inoculum for
subsequent fermentations; they can be stored for several days in
cold milk or water. (See also DAIRY PRODUCTS.)
kefiran See KEFIR.
Kellogg classification (of Neisseria gonorrhoeae) An early classification based on e.g.: (i) appearance of colony; (ii) autoagglutinability; and (iii) virulence. Types T1 and T2 correspond
to fimbriate, virulent strains, while types T3 and T4 correspond
to afimbriate, non-virulent strains.
keloidal blastomycosis Syn. LOBOMYCOSIS.
kelp (1) Any of various seaweeds that are used to obtain kelp
(sense 2). (2) The ashes obtained by burning various large brown
seaweeds such as Ascophyllum, Fucus, Laminaria, Macrocystis;
such ashes have been used as an agricultural fertilizer and as a
source of iodine, potash and soda (sodium carbonate).
KelseySykes test A CAPACITY TEST used to determine the
efficacy of each of several dilutions of a given disinfectant
under simulated practical conditions. (cf. USE-DILUTION TEST.)
To 3 ml of a given dilution of disinfectant is added a 1-ml
aliquot of bacterial suspension at times 0, 10 and 20 min; at
8, 18 and 28 min the disinfectant is subcultured to each of five
tubes of nutrient broth which are then incubated to detect the
presence or absence of viable bacteria. A given dilution passes
the test if no growth is obtained in at least two of the five
tubes inoculated from it at 8 and 18 min. The test organism
used is Pseudomonas aeruginosa NCTC 6749, Proteus vulgaris
NCTC 4635, Escherichia coli NCTC 8196 or Staphylococcus
aureus NCTC 4163; in a given test the organism used is that
which is the most resistant to the test disinfectant. To examine
the efficacy of the disinfectant under dirty conditions a yeast
Kineosporia
kidney stones (in humans) See UROLITHIASIS
kieselguhr Syn. DIATOMACEOUS EARTH.
kievitone An isoflavonoid PHYTOALEXIN produced by the French
bean (Phaseolus vulgaris). Cell-free extracts of Rhizoctonia
solani elicit high levels of kievitone from excised bean
hypocotyls, but those of Fusarium solani elicit only trace
amounts. Kievitone can be converted to the less fungitoxic kievitone hydrate by an extracellular enzyme produced by Fusarium
solani f.sp solani.
Kilham rat virus See PARVOVIRUS.
killed vaccine Syn. INACTIVATED VACCINE.
killer cells (immunol.) Commonly refers to NK CELLS (q.v.) but
may also refer e.g. to cytotoxic T cells.
killer factor Any of several protein toxins secreted by killer
strains of Saccharomyces cerevisiae and encoded by one of
two cytoplasmically co-inherited dsRNA elements; the K1 toxin
(formed by K1 or type 1 killer strains) binds initially to a
cell wall D-glucan of a sensitive cell and then transfers to the
cytoplasmic membrane where it disrupts the membrane potential.
One of the dsRNA elements (designated M) encodes both the
toxin and an immunity protein which confers on the producing
cell immunity to the toxin; the toxin contains two subunits, a
and b, both derived by proteolytic processing of a precursor
polypeptide during toxin secretion. The precursor polypeptide
apparently functions as the immunity protein possibly by
competing with the mature toxin for binding sites on the
membrane [Cell (1986) 46 105113]. The other dsRNA element
(designated L) encodes a protein required for the (separate)
encapsidation of M and L. The encapsidated particles (termed
VLPs: virus-like particles) are variously regarded as plasmids
or as viruses (Saccharomyces cerevisiae viruses, ScVs see
MYCOVIRUS). [Review: MR (1984) 48 125156.] (cf. KILLER
PLASMIDS; see also BACTERIOCIN.)
killer helper factor Syn. INTERLEUKIN-2.
killer paramecia Strains of Paramecium which are able to
kill other (sensitive) paramecia. See: CAEDIBACTER, LYTICUM,
MATE KILLER, PSEUDOCAEDIBACTER, R BODY, SPIN KILLING.
(cf. TECTIBACTER.)
killer plasmids (in yeasts) In some strains of Kluyveromyces
marxianus var. lactis the cells contain multiple copies of
each of two linear, cytoplasmically inherited dsDNA plasmids,
pGl1 and pGl2; cells containing these plasmids secrete a
glycoprotein toxin capable of killing other (sensitive) strains of
e.g. Candida, Kluyveromyces and Saccharomyces by inhibiting
adenylate cyclase activity. These plasmids can be transferred to
Saccharomyces cerevisiae (e.g. by protoplast fusion) on which
they confer the killer phenotype. [ARM (1983) 37 253276.]
(cf. KILLER FACTOR.)
killer yeasts See KILLER FACTOR and KILLER PLASMIDS.
kilobase See entry kb.
kimchi A Chinese and Korean food made by the lactic acid
fermentation of vegetables (usually cabbage or radishes). Preparation resembles that of SAUERKRAUT.
KinA, KinB See ENDOSPORE (sense 1).
kinase An ENZYME which catalyses the transfer of a phosphate group from one substrate (commonly ATP) to another;
examples include hexokinase and pyruvate kinase (both involved
in the EmbdenMeyerhofParnas pathway: see Appendix
I(a)), ADENYLATE KINASE, and PPi:phosphofructose dikinase (see
PYROPHOSPHATE).
Kineosporia A genus of bacteria (order ACTINOMYCETALES, wall
type I). The organisms form a substrate mycelium but no aerial
hyphae; sporangia, each containing one zoospore, develop on
kinesis
the hyphae. Growth occurs at/below 30 C, but not at 37 C. Type
species: K. aurantiaca.
kinesis (1) A behavioural response in which the speed (but not
the direction) of locomotion of a motile organism depends on
the intensity of an external stimulus; e.g., when light intensity
increases, an organism may swim faster (positive photokinesis)
or slower (negative photokinesis). (See also PHOTOTAXIS.) Kinesis, unlike TAXIS, is a continuous response and is not cancelled
by ADAPTATION.
(2) A behavioural response in which the rate of activity of an
organism depends on the intensity of an external stimulus. When
the activity concerned is speed of swimming, the phenomenon
is known as orthokinesis (syn. kinesis sense 1). When the
activity concerned is frequency of directional change, the
phenomenon is termed klinokinesis. [Photochem. Photobiol.
(1977) 26 559560.]
kinete A motile zygote, or a motile form derived from a zygote.
kinetic response Syn. KINESIS.
kinetid (ciliary corpuscle; kinetosomal territory) In ciliates: a
unit of the KINETY; it typically includes a CILIUM with its associated kinetosome, KINETODESMA, cytoplasmic membrane and
alveolus (see PELLICLE), and may also include e.g. a MUCOCYST,
PARASOMAL SAC and TRICHOCYST together with various microfibrils and/or microtubules (e.g. nematodesmata).
kinetin 6-Furfurylaminopurine, a compound formed during the
hydrolysis of DNA; it has CYTOKININ activity but it apparently
does not occur in plants.
kinetochore An electron-dense MICROTUBULE-ORGANIZING CENTRE, one of which develops on each side of the CENTROMERE
during MITOSIS.
kinetochore fibre See MITOSIS.
kinetocyst See AXOPODIUM.
kinetodesma (kinetodesmos) In some ciliates: one of a series of
overlapping endoplasmic fibrils which, by light microscopy, may
appear as a single fibre running parallel with, and to the right
of, a row of basal bodies in a somatic KINETY; each kinetodesma
arises from a kinetosome (near triplets 58, GRAIN CONVENTION),
passes a little to the right, and then runs anteriorly to terminate
in a position where it may overlap the kinetodesma(ta) of
the more anterior kinetosome(s). Kinetodesmata have crossstriations of periodicity ca. 30 nm. The role of the kinetodesmata
is unknown; they are commonly believed not to be involved in
ciliary coordination. (See also RULE OF DESMODEXY; SILVER LINE
SYSTEM.)
kinetofragments In many members of the KINETOFRAGMINOPHOREA: patches or short rows of kinetids (sometimes with
non-ciliferous kinetosomes) in the vicinity of the oral area; their
evolutionary origin is presumed to have been the anterior ends
of somatic kineties.
Kinetofragminophorea A class of protozoa (phylum CILIOPHORA) which characteristically have an apical or subapical
cytostome and a CYTOPHARYNGEAL APPARATUS which is usually
conspicuous; COMPOUND CILIATURE is typically absent, and ciliature in the oral region is not obviously differentiated from
that in other region(s) of the body. STOMATOGENESIS is typically
telokinetal (apparently apokinetal in the ENTODINIOMORPHIDA).
This class includes many of the ciliates previously referred to
as the lower holotrichs (e.g. the apostomes, chonotrichs, gymnostomes and trichostomes) together with e.g. the suctorians.
Subclasses: GYMNOSTOMATIA, HYPOSTOMATIA, SUCTORIA, VESTIBULIFERIA.
kinetoplast In protozoa of the KINETOPLASTIDA: a unique structure which forms a distinct region of the mitochondrion; it
Kluyveromyces
the thread-like molecules of DNA thus become more electrondense than the background. In a modification of this technique,
benzalkonium chloride is used instead of cytochrome c; since,
in this case, the DNA is not thickened with adherent protein, its
relationship to other macromolecules (e.g. polymerases) can be
determined more easily.
Klenow fragment (Klenow enzyme) The larger of two fragments obtained by proteolytic cleavage (using e.g. subtilisin) of
the DNA POLYMERASE I of Escherichia coli. The Klenow fragment
retains 5 -to-3 polymerase and 3 -to-5 exonuclease activities but
lacks 5 -to-3 exonuclease activity; it has various uses in genetic
engineering techniques and in DNA sequencing methods.
KlettSummerson colorimeter See TURBIDIMETRY.
Klett unit A unit of turbidity as measured with the KlettSummerson colorimeter using monochromatic light of a specified
colour.
Kliglers iron agar (KIA) A double-sugariron agar (cf. TSI
AGAR) used e.g. for distinguishing between members of the
Enterobacteriaceae. It is prepared as a slope with a deep butt,
and consists of nutrient agar (pH 7.4) supplemented with glucose
(ca. 0.1%), lactose (1%), sodium thiosulphate (0.05%), ferric
ammonium citrate (0.05%), and phenol red (ca. 0.0025%). In
general, bacterial reactions with KIA are similar to those with
TSI agar; however, the absence of sucrose in KIA means that
the lactose-negative reaction given by some organisms is not
masked by their ability to attack sucrose.
klinokinesis See KINESIS (sense 2).
Kloeckera
A genus of yeasts (class HYPHOMYCETES) which
have teleomorphs in the genus HANSENIASPORA. Vegetative cells
are more or less lemon-shaped (apiculate) and reproduce by
bipolar budding in basipetal succession; pseudomycelium may
be formed. All species ferment glucose; some ferment sucrose,
none ferments maltose (although some species can assimilate
maltose). NO3 is not assimilated. All species require inositol
and pantothenate for growth. Species (K. africana, K. apiculata,
K. apis, K. corticis, K. japonica, K. javanica) have been isolated
from fruit, soil, bark etc.
[Book ref. 100, pp. 873881.]
Klonostricha See HYPOTRICHIDA.
Klossiella See ADELEORINA.
Kluyver effect The phenomenon in which certain yeasts can
utilize particular disaccharides aerobically, but not anaerobically.
The mechanism underlying the effect is unknown [JGM (1982)
128 23032312].
Kluyvera
A genus of motile bacteria of the ENTEROBACTERIACEAE. MR +ve; VP ve; usually indole +ve and citrate +ve.
2-Oxoglutarate is formed from glucose. The organisms occur
in food, soil and sewage, and may be opportunist pathogens in
man. [Book ref. 22, pp. 511513.]
Kluyveromyces
A genus of yeasts (family SACCHAROMYCETACEAE) in which the cells are spheroidal, ovoid, ellipsoidal,
or cylindrical to elongate; vegetative reproduction occurs by
multilateral budding. Pseudomycelium may be formed. Asci
are evanescent; they contain one to many spores which may
be crescent-shaped, reniform, spheroidal etc, and which tend
to agglutinate after liberation. Cells contain ubiquinone-6 (Q6). All species can ferment glucose; K. marxianus var. lactis and some strains of K. marxianus var. marxianus can
ferment LACTOSE. NO3 is not assimilated. Eleven species
have been recognized primarily on the basis of hybridization
data; on this basis some former species (e.g. K. bulgaricus,
K. fragilis, K. lactis) have been relegated to varieties of
K. marxianus e.g., K. fragilis is K. marxianus var. marxianus (anamorph: Candida kefyr, = C. pseudotropicalis), and
k-MTs
field diaphragm. (v) Focus on the specimen with a low-power
(e.g. 10) objective, and adjust the substage condenser slightly
so that the edge of the field diaphragm is in sharp focus
in the plane of the specimen. (vi) Open the field diaphragm
until the small disc of light in the centre of the field of
view has expanded to cover the entire field. Under these conditions an image of the lamps filament is formed in the
lower focal plane of the substage condenser, and divergent
rays from each point of the filaments image pass through the
condenser and emerge as parallel rays which illuminate the
specimen.
koji A preparation consisting of mould (usually Aspergillus
oryzae) growing on cooked cereal and/or soybeans; the mould
produces enzymes (including a range of proteases, amylases,
pectinases, glutaminase, etc) and is used in the production of
e.g. SOY SAUCE and MISO.
The inoculum for making koji is a koji starter or tane koji : a
powder consisting of mould spores. Tane koji is typically made
by inoculating steamed polished rice with spores of selected
fungal strains; the rice is spread in shallow trays, incubated
at 30 C for ca. 5 days, and the spores are then harvested
and dried.
kojibiose A reducing disaccharide: a-D-glucopyranosyl-(1 2)D-glucopyranose. It can occur e.g. as a product of enzymic
degradation of certain plant carbohydrates, and is present in
glycerol TEICHOIC ACIDS of group D streptococci (in which it
is linked to the C-2 position of glycerol and may be esterified
with D-alanine).
kojic acid (5-hydroxy-2-hydroxymethyl-4-pyrone) A secondary
metabolite produced e.g. by Aspergillus spp (particularly the
flavusoryzae group) when grown on glucose, xylose or certain
other sugars. It is a chelating agent which gives a strong
blood-red colour with Fe3+ ; it also has weak antibiotic activity
(enhanced by certain metal ions), being effective mainly against
Gram-negative bacteria.
Kolmer CFT See STANDARD TESTS FOR SYPHILIS.
Kolpoda Syn. COLPODA.
kombu See LAMINARIA.
Konservomat See BATCH RETORT.
Kopeloff modification A modification of the GRAM STAIN used
for staining anaerobic bacteria. The technique involves the
addition of ca. 5 drops of NaHCO3 solution (5%) to the smear
after the latter has been flooded with crystal violet (1%); the
iodine solution (iodine 2%, KI 0.1%) includes NaOH (0.4%),
decolorization is carried out with acetonealcohol, and safranin
(2%) is used for counterstaining.
Kopliks spots Small, white, necrotic lesions formed in the
mouth in the early stage of MEASLES.
Kordyana See EXOBASIDIALES.
Korean haemorrhagic fever (epidemic haemorrhagic fever) A
VIRAL HAEMORRHAGIC FEVER involving renal dysfunction, proteinuria and oliguria; the mortality rate may be up to 30%. The
causal agent is the Hantaan virus (see HANTAVIRUS); reservoirs
of infection are found in rodent populations. Infection typically occurs by inhalation of aerosols of urine, faeces etc. from
infected rodents. The disease occurs in Asia and Europe.
Korfia See HELOTIALES.
Kornberg enzyme See DNA POLYMERASES.
Koserella A genus of Gram-negative bacteria of the ENTEROBACTERIACEAE. K. trabulsii (formerly known as enteric group 45
and originally identified as an atypical strain of Hafnia alvei )
has been isolated from clinical specimens; it is MR +ve; VP
ve; indole ve; citrate +ve; H2 S ve; urease ve; LDC
Kyzylagach virus
+ve; ODC +ve; and it produces acid from cellobiose and melibiose but not from glycerol, lactose or sucrose. [JCM (1985) 21
3942.]
Kosers citrate medium A medium, used for the CITRATE TEST,
containing (per 100 ml of water): NaCl (0.5 g), MgSO4 7H2 O
(0.02 g), (NH4 )H2 PO4 (0.1 g), K2 HPO4 (0.1 g), citric acid
(0.2 g); pH 6.8.
Kosters stain A stain for detecting Brucella spp in mammalian
tissues. The smear or section is stained for 1 min in a solution
made by mixing saturated aqueous safranin and normal KOH
(2:5 v/v); the slide is then washed in tap water and differentiated in 0.1% sulphuric acid (two changes for a total period
of 1020 sec). The slide is washed in tap water and counterstained with 1% carbol methylene blue. Brucella stains orange,
tissues blue.
Kotonkan virus See LYSSAVIRUS.
koumiss (kumiss) An acidic, mildly alcoholic, fermented milk
beverage made in the former USSR. Traditionally made from
mares milk, it is now also made from cows milk. Organisms
involved in the fermentation include Lactobacillus bulgaricus
(the main acid-producer) and lactose-fermenting yeasts; the main
products of fermentation are lactic acid, ethanol and CO2 . (See
also DAIRY PRODUCTS.)
Kovacs indole reagent An INDOLE TEST reagent: p-dimethylaminobenzaldehyde (5 g) is dissolved in 75 ml amyl (or
isoamyl) alcohol, and conc. HCl (25 ml) is slowly added; it
is stored at 4 C in the dark.
Kovacs oxidase reagent A 1% aqueous solution of tetramethylp-phenylenediamine dihydrochloride. (See also OXIDASE TEST.)
kPa 103 Pa (see PASCAL).
KpnI See RESTRICTION ENDONUCLEASE (table).
krad 103 rad (see RAD).
kraft pulps See PAPER SPOILAGE.
Krebs cycle Syn. TCA CYCLE.
Krebspest Syn. CRAYFISH PLAGUE.
Kruses bacillus Archaic name for Shigella sonnei (Kruses
Bacillus pseudodysenteriae type E).
Kudoa See MYXOSPOREA.
kumiss Syn. KOUMISS.
Kunin antigen Syn. ENTEROBACTERIAL COMMON ANTIGEN.
Kunjin virus See FLAVIVIRIDAE.
Kupffer cells Actively phagocytic cells which line the liver sinusoids.
Kurthia
A genus of Gram-positive, asporogenous, catalasepositive, obligately aerobic bacteria which occur e.g. in meat
and meat products. In the exponential growth phase the organisms occur in long chains of rods (or of short filaments) but
in the stationary phase coccoid forms or short rods predominate; individual rods are peritrichously flagellated. Kurthia
spp are chemoorganotrophs which can utilize certain alcohols
(e.g. ethanol, ethanediol), amino acids (e.g. L-alanine) and fatty
acids (e.g. butyric acid). VP ve. Indole-negative. The type
species, K. zopfii, grows in the temperature range 535 C and is
killed by heating to 55 C/20 minutes. K. gibsonii grows in the
range 545 C and survives heating to 55 C/20 minutes [SAAM
(1983) 4 253276]. GC%: ca. 3638.
kuru A human TRANSMISSIBLE SPONGIFORM ENCEPHALOPATHY
[early description: NEJM (1957) 257 974978]. The incubation
period may range from a few years to some 30 years or
more; characteristically there is ataxia, tremor, dysarthria and
sometimes late dementia, and death occurs within a year of
the onset of symptoms. Kuru is found in certain regions of
Papua New Guinea and is believed to result from the ingestion
of prion-containing flesh during ritual cannibalism; as this
practice has declined, the incidence of kuru has decreased.
Kuru can be transmitted experimentally to chimpanzees and to
other primate and non-primate animals; goats (but not sheep)
inoculated with tissue from kuru victims develop a disease that
closely resembles SCRAPIE. [Review of kuru: Book ref. 159,
pp. 483544 (497510).]
Kusnezovia
A genus of poorly-characterized, manganesedepositing bacteria found in mud; the organisms have not been
obtained in pure culture, and the validity of the genus (and of
an apparently similar genus, Caulococcus) has been questioned
[Book ref. 45, pp. 529530].
Kyasanur Forest disease An acute, tick-borne human disease
(vector: mainly Haemaphysalis sp) caused by a flavivirus (see
FLAVIVIRIDAE); it occurs in Mysore State, India. Onset is sudden,
with e.g. fever, headache, severe myalgia, haemorrhages, etc.
Mortality rates are generally low (<5%). Monkeys may act as
a reservoir of infection.
Kyzylagach virus See ALPHAVIRUS.
419
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
L
The vegetative stage of the organism consists of spindleshaped cells which produce a branching, anastomosing network
of membrane-enclosed slime-ways (variously called the ectoplasmic net, filoplasmodium, net plasmodium, rhizoplasmodium,
etc); the cells move (by gliding) within these slime-ways. The
vegetative cells contain a characteristic organelle, the sagenogenetosome or sagenogen (formerly bothrosome), which is
apparently involved in the production of the ectoplasmic net
and possibly also in the movement of the cells through the net.
The cells feed osmotrophically; enzymes are secreted from the
ectoplasmic net, and the soluble products of digestion diffuse
back to the cells within the net.
In at least some labyrinthulas biflagellate zoospores are
formed, each bearing one anteriorly directed tinsel flagellum
and one posteriorly directed whiplash flagellum; an orange
eyespot occurs at the base of the flagellar apparatus. The
zoospores are haploid, their formation involving meiosis. They
apparently develop directly into spindle-shaped cells; copulation
is presumed to occur between two of these cells.
labyrinthulids See LABYRINTHULAS.
Labyrinthulina See GYMNOMYXA.
Labyrinthuloides See THRAUSTOCHYTRIDS.
Labyrinthulomycetes A class of organisms (division MYXOMYCOTA) which includes the LABYRINTHULAS and the THRAUSTOCHYTRIDS; these organisms are apparently unrelated to other
members of the Myxomycota.
lac operon (lactose operon) An OPERON containing genes which
encode proteins involved in the uptake and utilization of bgalactosides such as LACTOSE. The lac operon occurs e.g. in
Escherichia coli in which it is located at ca. 8 minutes on
the chromosome map. A simplified scheme for the lac operon
is shown in the figure. The lacZ gene encodes b-galactosidase,
lacY encodes a transport protein, b-galactoside permease, and
lacA encodes thiogalactoside transacetylase. (LacA catalyses the
transfer of an acetyl group from acetyl-CoA to a b-galactoside.
Its function in vivo is unknown; it has been suggested that it may
be involved in the detoxification of non-metabolizable sugars by
bringing about their acetylation and, hence, excretion.)
According to an earlier view, control of the lac operon
(illustrated in the figure) is as follows. In the absence of an
inducer, the regulator protein (repressor), which is active in
tetramer form, binds tightly to the OPERATOR. The operator (O)
is a region of ca. 16 bp which occurs immediately downstream
of the promoter (P); the operator is an imperfect PALINDROMIC
SEQUENCE centred at about nucleotide +10 in relation to the
transcription start site (see PROMOTER). The binding of repressor
to the operator reduces transcription to a minimal level (only a
few molecules of product being produced per cell).
If an inducer (ALLOLACTOSE or e.g. IPTG) is present, it binds to
the operator-bound repressor and causes the repressor to undergo
a conformational change that reduces its affinity for the operator;
the repressor then detaches from the operator, and the level of
lacZYA transcription increases rapidly; up to ca. 10000 molecules
of b-galactosidase may appear in the cell within minutes of
induction. (The presence of inducer does not necessarily lead
to expression of the lac operon: see CATABOLITE REPRESSION.)
While the above description gives the essential mode of
control of the lac operon, the actual process is rather more
complex [Mol. Microbiol. (1992) 6 24192422]. Thus, in
lac operon
(a)
DNA
lac I
lac Z
lac Y
lac A
RNA
polymerase
mRNA
protein
regulator
protein
(b)
DNA
lac I
lac Z
lac Y
lac A
mRNA
RNA
polymerase
protein
inactive
regulator
inducer
(allolactose) inducer
complex
b-galactosidase
b-galactoside
permease
thiogalactoside
transacetylase
THE lac OPERON in Escherichia coli (a simplified scheme). The lac operon consists of (i) three regulated genes: lacZ, lacY and lacA (see entry);
(ii) a promoter (P); (iii) an operator (O); and (iv) the regulator gene, lacI, encoding a repressor. lacI is transcribed constitutively, at a low rate,
from its own independent promoter.
(a) In the absence of an inducer, the regulator protein (LacI) binds to the operator, O, and minimizes transcription of genes lacZ, lacY
and lacA by the RNA polymerase (seen here at the promoter); there is some leakage: a few molecules of product are formed under these
conditions in each cell.
(b) In the presence of lactose (taken up by protonlactose symport), b-galactosidase converts some of the lactose to allolactose, the inducer
of the lac operon. Allolactose binds to, and inactivates, the regulator protein which dissociates from the operator, thus permitting transcription
and translation of the regulated genes. (The single mRNA transcript contains an initiator codon and a stop codon for each of the three genes.)
When all the lactose has been metabolized, transcription of the lac operon is no longer needed; the inducer (allolactose) is no longer formed,
and the (now active) regulator protein represses the operon.
The lac operon is subject to CATABOLITE REPRESSION (q.v.).
See entry for further details.
Reproduced from Bacteria, 5th edition, Figure 7.11, page 138, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN
0471-98880-4) with permission from the publisher.
Lac plasmid
wild-type; in these cells, a defective (mutant) repressor subunit
can interact with wild-type subunits to form a defective tetramer
(an example of negative complementation).
Mutants designated lacI s produce a super-repressor which
retains its affinity for the operator but has negligible affinity for
the inducer the repressor remains tightly bound to the operator
even in the presence of inducer (i.e. the operon is non-inducible),
and the defect cannot be overcome by the presence of normal
repressor (i.e. the mutant phenotype is dominant).
A mutation in the operator may reduce the affinity of the
operator for the repressor; such mutants (designated lacO c or
oc ) express the lac genes constitutively, and the oc allele exhibits
CIS-DOMINANCE.
Lac plasmid Syn. LACTOSE PLASMID.
lacA gene See LAC OPERON.
laccase A monophenol oxidase (EC 1.14.18.1). Many basidiomycetes (and some ascomycetes and deuteromycetes) produce
extracellular laccase which appears to be involved in the
degradation of LIGNIN and e.g. in the induction of basidiocarp
development [JGM (1982) 128 27632770]. Most or all fungal
laccases are copper-containing blue proteins which can oxidize
o- and p-phenols and aromatic amines.
Lachnospira
A genus of bacteria (family BACTEROIDACEAE)
which occur e.g. in the bovine RUMEN. Cells: curved rods,
0.40.6 2.04.0 m, with one lateral or subpolar flagellum
per cell; the cells from young cultures may give a weak Grampositive reaction, while those from older cultures may stain
Gram-negatively. Glucose fermentation yields acetate, ethanol,
formate, lactate, CO2 and H2 ; these products, together with
methanol, are also formed from pectin fermentation. Butyrate,
propionate and succinate are not formed. Growth is flocculent in
glucoserumen fluid media. Type species: L. multiparus. [Book
ref. 22, pp. 661662.]
lachrymal canaliculitis Inflammation of the lachrymal ducts
and adjacent tissues, together with the formation of yellowish
concretions within the ducts; the disease is non-invasive, usually
mild, and the causal agent is commonly Arachnia propionica or
Actinomyces israelii.
laciniate Lobed or notched.
lacrimoid (lacrioid) Shaped like a tear-drop.
Lacrymaria See GYMNOSTOMATIA.
lactacin A See BACTERIOCINS.
lactacin B See BACTERIOCINS.
lactacin F See BACTERIOCINS.
b-lactam antibiotics A family of ANTIBIOTICS, each of which
contains the b-lactam ring (see figure). CEPHALOSPORINS and
PENICILLINS are produced by fungi, while the more recently
discovered members (see CARBAPENEMS, CLAVAMS, MONOBACTAMS, NOCARDICINS) are produced by bacteria [carbapenems and
clavams: TIM (1998) 6 203208]; synthetic and semi-synthetic
members have been manufactured. Most b-lactam antibiotics are
antibacterial, but some of the newer ones are antifungal. As well
as possessing weak or moderate antibacterial activity, CLAVULANIC ACID and many CARBAPENEMS also inhibit b-LACTAMASES
(see also b-LACTAMASE INHIBITOR).
The antibacterial action of penicillins and cephalosporins
has been widely studied in Escherichia coli. One of the
earliest proposals was that penicillin acted as an analogue
of D-alanine D-alanine, thus inhibiting the cross-linking of
PEPTIDOGLYCAN with resultant lysis of the structurally weakened
cells. The b-lactam antibiotics are now known to have multiple
killing sites, and various PENICILLIN-BINDING PROTEINS (PBPs)
have been identified as lethal targets. In many cases a given blactam antibiotic has a roughly similar degree of affinity for more
b-lactamases
dihydrothiazine
ring
b-lactam
ring
thiazolidine
ring
b-lactam
ring
H
H
R
CH3
penicillin
amidase
6
7
S
1
CH3
5
4
COOH
CH2R
b-lactamase
b-lactamase
(a)
COOH
(b)
H
R
OH
N
H
N
N
O
C
COOH
(c)
(d)
oxazolidine
ring
R
N
O
OH
COOH
(e)
2
3
COOH
(f)
b-LACTAM ANTIBIOTICS. (a) Penicillin nucleus. In 6-aminopenicillanic acid (6-APA): R = H. (b) Cephalosporin nucleus. In 7aminocephalosporanic acid (7-ACA): R = H, R = O.CO.CH3 ; in cephalosporin C: R = CO.(CH2 )3 .CHNH2 .COOH, R = O.CO.CH3 .
(c) Nocardicin nucleus. (d) Monobactam nucleus. (e) Carbapenem nucleus. (f) Clavulanic acid (a clavam).
Lactarius
The LDV genome is a single molecule of positive-sense
ssRNA, and the virus has been placed in the arterivirus group
(see ARTERIVIRUS).
LDV replicates only in a particular subset of MACROPHAGES,
the macrophages being destroyed in the process. [Determinants
of macrophage susceptibility: JGV (1985) 66 14691477.]
Infection results in a persistent viraemia (maintained by the
ongoing production of new susceptible cells) and gives rise to
elevated levels of certain plasma enzymes particularly certain
(positively charged) lactate dehydrogenase isoenzymes. Elevated
levels of these enzymes result from their reduced rates of
clearance from the plasma; such enzymes may be cleared in the
normal mouse by the particular subset of macrophages destroyed
by LDV.
Infected mice generally show little sign of disease, but they
exhibit slight splenomegaly and disturbances in the immune
system (altering the growth of tumours, response to infection etc.). In the acute phase of infection there is transient
polyclonal activation of antibody-producing cells resulting in
increased immunoglobulin levels and transient depression of
cell-mediated immunity; in the chronic phase, the humoral
response is depressed, while cell-mediated immunity returns to
normal. Antibodies to LDV are produced, and virusantibody
complexes circulate in the blood; the immune complexes
cause little tissue reaction possibly because they do not bind
complement. LDV can apparently cause age-dependent polioencephalomyelitis (resulting in paralysis) in certain strains of
mouse.
LDV is apparently transmitted by blood-sucking parasites and
by fighting; transplacental transmission can occur if the mother
becomes infected during pregnancy or lactation, but generally
does not occur in chronically infected mothers.
[LDV (review): JGV (1985) 66 22972312.]
lactic acid (CH3 .CHOH.COOH) A compound present e.g. in
many fermented DAIRY PRODUCTS, and also widely used as a food
additive. Only the L(+)-isomer can be readily assimilated by man
and animals. L(+)-Lactic acid is obtained commercially by the
LACTIC ACID FERMENTATION of sucrose by LACTIC ACID BACTERIA;
it is used primarily in the food industry, being added e.g. to
confectionary, pickles, beverages, etc [AvL (1983) 49 86].
lactic acid bacteria A (non-taxonomic) group of Gram-positive,
non-sporing bacteria which carry out a LACTIC ACID FERMENTATION of sugars; it includes species of Lactobacillus, Lactococcus,
Leuconostoc and Pediococcus. (Bifidobacterium is sometimes
included.)
Lactic acid bacteria are used extensively in the food industry
(e.g. BREAD-MAKING (sourdough), DAIRY PRODUCTS, SALAMI);
however, they can also cause food spoilage (see e.g. MEAT
SPOILAGE; cf MALOLACTIC FERMENTATION). (See also SILAGE.)
Lactic acid bacteria are nutritionally fastidious and weakly
proteolytic [for proteolytic systems see AvL (1983) 49
225245]. Many activities of the lactic acid bacteria (e.g. LACTOSE metabolism) appear to be plasmid-linked [AvL (1983) 49
259274].
Although lactic acid bacteria are primarily fermentative, many
strains can grow in the presence of air and can carry out
certain oxidation reactions using flavin-containing oxidases,
peroxidases, or NAD-independent dehydrogenases oxidizing
at least some of the pyruvic and lactic acids (formed by
fermentative pathways) to acetic acid and carbon dioxide [AvL
(1983) 49 209224]. (See also LEUCONOSTOC.) The hydrogen
peroxide formed during these oxidations has some preservative
action in fermented foods (see FOOD PRESERVATION (e)).
Lactobacillus
and prevent its translation. [Improvement and optimization of
two engineered phage-resistance mechanisms in Lactococcus
lactis: AEM (2001) 67 608616.]
lactic acidosis (vet.) See ACIDOSIS (1).
lactic dehydrogenase virus Syn. LACTATE DEHYDROGENASE VIRUS.
lacticin 3147 A pore-forming LANTIBIOTIC produced by Lactobacillus lactis subsp lactis. It consists of two peptide components, both of which are needed for activity; each component
requires modification by a separate enzyme [Microbiology
(2000) 146 21472154]. In sensitive cells, the lesions formed
by lacticin 3147 are ion-specific pores.
A lacticin 3147-producing starter culture has been tested for
its ability to inhibit Listeria monocytogenes in the manufacture
of cottage cheese [JAM (1999) 86 251256].
lactiferous hyphae See LACTARIUS.
Lactobacillaceae A family of bacteria (sole genus: LACTOBACILLUS). [Book ref. 21, p. 576.]
Lactobacillus A genus of Gram-positive, asporogenous bacteria
which are anaerobic, microaerophilic, or facultatively aerobic.
Cells are rods or coccobacilli, occurring singly or in chains.
Most strains are non-motile. Catalase ve, but may be catalase +ve in haem-containing media. Metabolism is predominantly fermentative, lactic acid being formed from glucose
either homofermentatively or heterofermentatively. (See LACTIC
ACID BACTERIA.) Species are commonly aciduric or acidophilic.
Nutritional requirements are complex, generally including carbohydrates, peptones, vitamins etc. Lactobacilli may be grown
e.g. on APT agar; growth is stimulated by Tween 80.
The genus (GC%: ca. 3253) is divided into three subgenera: Betabacterium, Streptobacterium and Thermobacterium.
Betabacteria carry out HETEROLACTIC FERMENTATION of glucose
(and hence require thiamine and produce CO2 from glucose);
fructose is fermented and can be reduced to mannitol (see e.g.
SILAGE), and PENTOSES may be fermented. Streptobacteria and
thermobacteria carry out HOMOLACTIC FERMENTATION of glucose
(CO2 not produced, thiamine not required); fructose is usually
fermented but it cannot be reduced to mannitol. Streptobacteria can grow at 15 C (and may or may not grow at 45 C),
can ferment pentoses, and produce CO2 from gluconate. Thermobacteria can generally grow at or above 45 C but not at 15 C,
and cannot ferment pentoses or produce CO2 from gluconate.
Species are distinguished by biochemical tests. The nature of
the lactic acid produced can be a useful criterion: betabacteria produce DL-lactic acid, streptobacteria and thermobacteria
produce (mainly) L(+)-, D()- or DL-lactic acid, according to
species. Betabacteria include e.g. L. brevis, L. buchneri (possibly a subspecies of L. brevis), L. cellobiosus, L. confusus,
L. desidiosus, L. fermentum, L. hilgardii, L. viridescens; streptobacteria include e.g. L. alimentarius, L. casei, L. coryniformis,
L. curvatus, L. farciminis, L. plantarum, L. xylosus (cf. LACTOCOCCUS); thermobacteria include e.g. L. acidophilus, L. bulgaricus, L. delbrueckii (type species of the genus), L. helveticus,
L. lactis, L. leichmannii, L. ruminis, L. salivarius. [Book ref. 46,
pp. 16531679.] (L. bifidus: see BIFIDOBACTERIUM.) [Classification of L. bulgaricus, L. lactis and L. leichmannii as subspecies
of L. delbrueckii : SAAM (1983) 4 552557.]
Lactobacilli are found e.g. in man and animals (see
e.g. DENTAL CARIES, GASTROINTESTINAL TRACT FLORA, VAGINA
MICROFLORA), in MILK, DAIRY PRODUCTS and other fermented
foods and beverages (see e.g. sourdough BREAD-MAKING, PULQUE,
SOY SAUCE), and usually in very small numbers on plant
material (see e.g. SILAGE, PICKLING). (See also BEER SPOILAGE,
MALOLACTIC FERMENTATION, MEAT SPOILAGE, MILK SPOILAGE, WINE
lactocin 27
bacteriostatic against Gram-positive, catalase-negative bacteria
(e.g. streptococci and lactobacilli).
The LP system has a potential application in the preservation
of (refrigerated or uncooled) milk; for this purpose, levels
of H2 O2 in the milk could be boosted e.g. by the addition
of a glucose/glucose oxidase H2 O2 -generating system and (if
necessary) SCN . Components which activate the LP system
have been incorporated into an anti-plaque toothpaste to inhibit
oral streptococci (see DENTAL CARIES).
[Review: J. Food Protect. (1984) 47 724732.]
lactophenol cotton blue A general mycological MOUNTANT and
DYE. Phenol (20 g), water (20 ml), lactic acid (20 ml), and
glycerol (30 ml) are warmed together, and cotton blue (0.05 g)
is added.
lactose A disaccharide (b-D-galactopyranosyl-(1 4)-D-glucopyranose) present in MILK. Lactose is the major source of carbon
and energy for LACTIC ACID BACTERIA growing in milk (see also
LACTIC ACID FERMENTATION). The ability to metabolize lactose is
an important characteristic in the identification of members of
the family Enterobacteriaceae.
In Escherichia coli and other enterobacteria, and in most lactobacilli (though not Lactobacillus casei ), lactose is generally
taken up by a lactose-specific proton symport TRANSPORT SYSTEM; the lactose is then split into glucose and galactose by
b-galactosidase (see also LAC OPERON), the glucose and galactose
being metabolized via the EMP and Leloir pathways, respectively: see Appendix III(a).
In e.g. Lactobacillus casei, Lactococcus lactis and Staphylococcus aureus, lactose is taken up by a PEP-dependent phosphotransferase system (see PTS) entering the cell as lactose
phosphate (apparently as lactose bisphosphate in L. lactis [Book
ref. 11, pp 196203]) which is then hydrolysed by phosphob-D-galactosidase (P-b-gal); the glucose (glucose 6-phosphate
in L. lactis) and galactose 6-phosphate moieties are metabolized via the EMP and D-tagatose 6-phosphate pathways,
respectively see Appendix III(a). In at least some strains of
L. lactis, all the enzymes for lactose metabolism from transport to the formation of triose phosphates via the D-tagatose 6phosphate pathway appear to be plasmid-encoded [JB (1983)
153 7683]; strains lacking the lactose plasmid can metabolize
lactose via the permease/b-galactosidase mechanism and Leloir
pathway, but their rates of lactose metabolism and growth are
much reduced (cf. LACTIC ACID STARTERS).
In yeasts, Kluyveromyces marxianus var. lactis and var. marxianus (some strains) are among the few capable of fermenting
lactose (see SINGLE-CELL PROTEIN); however, other yeasts may be
able to metabolize lactose oxidatively (cf. KLUYVER EFFECT).
lactose killing Lactose-mediated SUBSTRATE-ACCELERATED DEATH.
lactose operon Syn. LAC OPERON.
lactose plasmid (Lac plasmid) A PLASMID which specifies the
uptake and metabolism of LACTOSE. Conjugative lactose plasmids
occur e.g. in some lactococci.
lacunose Covered with pits or indentations.
lacY gene See LAC OPERON.
lacZ gene See LAC OPERON.
LAD LEUKOCYTE ADHESION DEFICIENCY.
Laemmli electrophoresis Syn. SDS-PAGE.
laeoplectic metachrony See METACHRONAL WAVES.
Laetiporus See APHYLLOPHORALES (Polyporaceae).
laevulose D-Fructose.
LAF See INTERLEUKIN-1.
lag phase (of growth) See BATCH CULTURE.
Lagarde retort An airsteam BATCH RETORT.
426
Lampropedia
e.g. in Coprinus spp; they are rectangular in transverse crosssection (opposite faces of the lamella being parallel), and the
basidia at the lower (free) end reach maturity before those higher
up the lamella. (See also BASIDIOSPORES.)
lamellate (mycol.) Having lamellae (see LAMELLA).
lamina (algol.) Syn. BLADE.
laminaran Syn. LAMINARIN.
Laminaria A genus of large marine algae (division PHAEOPHYTA)
which exhibit a heteromorphic ALTERNATION OF GENERATIONS.
The sporophyte is a large blade with a stipe and holdfast;
growth occurs at the region between stipe and blade, and at the
MERISTODERM. The gametophyte is a microscopic filamentous
structure. L. japonica is used as a food in China (where it is
called haidai) and e.g. in Japan (kombu) [Book ref. 130,
pp. 688690]. (See also ALGINATE.)
laminaribiose A reducing disaccharide: b-D-glucopyranosyl(1 3)-D-glucopyranose.
laminarin (laminaran) The storage polysaccharide characteristic
of members of the Phaeophyta. Laminarins are essentially
linear (1 3)-b-D-glucans in which the chains may terminate
with D-mannitol (M-chains, non-reducing) or with D-glucose
(G-chains, reducing); low levels of branching via (1 6)b-glucosidic linkages may occur. Laminarins from different
sources vary in their mannitol content (usually ca. 24%),
degree of branching, and average chain length. [Book ref. 37,
pp. 481486.] Laminarins may be attacked e.g. by certain fungi
and by Nocardia spp. (cf. CHRYSOLAMINARIN.)
lamivudine ()2 -deoxy-3 -thiacytidine: an ANTIVIRAL AGENT
with activity against the hepatitis B virus; this nucleoside
analogue inhibits the viral DNA polymerase, thus inhibiting
viral replication. As a candidate therapeutic agent, lamivudine
was able significantly to reduce serum levels of viral DNA in
phase III clinical trials. However, resistance to the drug may
appear during long-term treatment programmes; such resistance
has been found to be associated with mutant forms of the
polymerase. [PCR-based detection of mutant strains of HBV
with reduced susceptibility to lamivudine: JCM (1999) 37
33383347.]
Lamivudine is also an ANTIRETROVIRAL AGENT which acts as
a NUCLEOSIDE REVERSE TRANSCRIPTASE INHIBITOR; it is one of the
drugs used against AIDS.
Lampit See CHAGAS DISEASE.
Lamprene CLOFAZIMINE.
Lamprocystis
A genus of photosynthetic bacteria (family
CHROMATIACEAE). Cells of the sole species, L. roseopersicina,
are motile cocci, 33.5 m, which contain Bchl a, various
carotenoids (cell suspensions are typically purple), and gas vacuoles. L. roseopersicina is a strict anaerobe which requires sulphide and vitamin B12 .
Lamproderma See MYXOMYCETES.
Lampropedia
A genus (incertae sedis) of aerobic, oxidasepositive, catalase-positive, chemoorganotrophic, Gram-negative
bacteria which have been isolated e.g. from stagnant and polluted waters. Cells: non-flagellated, non-pigmented, rounded
to cuboid, ca. 1.01.5 1.02.5 m, which occur in thin,
hydrophobic sheets (on liquid and solid media) each sheet
consisting of a number of roughly square tablets of 1664
cells arranged, with sides adjacent, in the same plane; cell division occurs synchronously. Metabolism: respiratory (oxidative).
Carbon and energy sources include TCA cycle intermediates;
carbohydrates are not used. Optimum growth temperature: 30 C.
GC%: ca. 61. Type species: L. hyalina.
[Book ref. 22, pp. 402406.]
LAMPs
(convexities in the upper surface corresponding to hollows in the
lower surface); asci contain one or two large spores (those of
Umbilicaria contain 8 smaller spores). (L. pustulata: formerly
U. pustulata.)
lasalocid A MACROTETRALIDE antibiotic which is used as an anticoccidial agent in poultry, and which has been used as a FEED
ADDITIVE for ruminants (its mode of action apparently being
similar to that of MONENSIN).
Lassa fever A VIRAL HAEMORRHAGIC FEVER caused by the Lassa
virus (see ARENAVIRIDAE); it occurs in Africa, especially Nigeria,
Liberia and Sierra Leone. Early symptoms resemble those of
other VHFs; petechiae may be present, and there is marked
pharyngitis with white patchy exudate adhering to the soft
palate and pharyngeal region. In fatal cases death usually occurs
during the second week of infection; mortality rates may be
3066% among hospital cases, but subclinical infections may
occur. The natural reservoir of the virus is the multimammate
rat Mastomys natalensis. Human infection may occur e.g. by
contamination of wounds with urine from infected rats; personto-person transmission also occurs.
Lassa virus See ARENAVIRIDAE and LASSA FEVER.
latamoxef Syn. MOXALACTAM.
late blight (of potato) A POTATO DISEASE caused by Phytophthora
infestans (see PHYTOPHTHORA). Dark patches appear on the upper
surfaces of leaves (and sometimes on stems), and patches of
white mildew (sporangium-bearing sporangiophores) develop
on corresponding regions on the undersides of leaves. Disease
may spread rapidly from plant to plant. Tubers develop dark
surface patches and succumb to a dry brown rot and sometimes
to a secondary soft rot. Protectants used against late blight
include e.g. MANEB and ZINEB. Late blight was responsible for
the Irish potato famine in the 1840s.
[Review: Book ref. 58, pp. 317.]
late genes See VIRUS.
latent infection (1) (animal virol.) An asymptomatic infection in
which infectious virions are not produced. (See PERSISTENCE.)
(2) (plant virol.) Any viral infection in which symptoms do
not occur whether or not virus replication occurs.
latent period See ONE-STEP GROWTH EXPERIMENT.
latent virus A virus which can establish a LATENT INFECTION
(sense 1 or 2).
lateral body (virol.) See POXVIRIDAE.
lateral transmission See HORIZONTAL TRANSMISSION.
laterosporolysin See THIOL-ACTIVATED CYTOLYSINS.
latex (1) A product of the rubber tree, Hevea brasiliensis. Natural
latex is a colloidal suspension of polyisoprenoid particles in
an aqueous phase containing e.g. carbohydrates and proteins;
it is readily attacked by a variety of microorganisms. (See also
RUBBER SPOILAGE.)
(2) See LATEX PARTICLE TEST.
(3) See LACTARIUS.
latex particle test (latex test) (serol.) A PASSIVE AGGLUTINATION
test in which antibody or soluble antigen is adsorbed to particles
of a synthetic latex: e.g. a suspension of particles of polystyrene
(commonly ca. 0.81 m diam.), a substance to which proteins
tend to adsorb.
For example, to detect antibodies to a given antigen, antigencoated particles of latex are exposed to the patients serum; the
presence of homologous antibodies in the serum is indicated by
agglutination of the latex particles (which are bound together
by antigenantibody bridges). Uncoated particles of latex, and
known negative serum, are used for controls.
Latex particle tests have a wide range of uses, being able not
only to detect serum antibodies and soluble antigens but also to
LCR
LCR Ligase chain reaction: a PROBE-based method for copying
(amplifying) a given sequence of nucleotides in DNA; like
PCR (but unlike NASBA or SDA), LCR involves thermal cycling.
Essentially, sample DNA is heat-denatured in order to expose the
target sequence (amplicon) in one strand and its complementary sequence in the other strand; on lowering the temperature,
two oligonucleotide probes bind (anneal ) in adjacent positions
to cover the entire amplicon while another two probes bind
to the amplicons complementary sequence. If a given pair of
probes binds correctly to the target, the 5 terminus of one probe
will abut the 3 terminus of the other; when this occurs, a
covalent link can be made between the 5 and 3 termini by
a heat-stable DNA LIGASE. A pair of ligated probes will thus form
a copy of the target sequence and can be used as a target (by
other probes) in the subsequent rounds of amplification. Ligation
and amplification of the sequence-specific probes argues for the
presence of the given target sequence in the sample DNA.
Note that, for ligation to occur, both juxtaposed bases in
a given pair of probes must base-pair correctly with the
corresponding nucleotides in the template strand (even if mismatches occur elsewhere in the probetarget duplex); moreover,
the 5 end of one probe must be phosphorylated in order for
ligation to occur.
Commercial LCR-based assays (LCx assays; Abbott Diagnostics) are used to detect specific sequences of DNA from certain pathogens in clinical specimens; such assays include tests for
Chlamydia trachomatis, Neisseria gonorrhoeae and Mycobacterium tuberculosis. These assays differ from the (basic) format
described above. Thus, the two probes in a bound pair are separated by a gap of one to several nucleotides. Consequently,
part of each cycle includes a period of extension, from the 3
end of one probe, by a DNA polymerase present in the reaction mixture; closure of the gap is followed by ligation. Cycling
thus involves three phases of temperature; in the Abbott LCx
assay for Chlamydia trachomatis, these phases are: (i) 93 C for
denaturing the dsDNA sample, (ii) 59 C for annealing, and (iii)
62 C for extension/ligation. Corresponding values in the LCx
assay for M. tuberculosis are (i) 94 C, (ii) 64 C and (iii) 69 C.
An amplification of at least 10 million-fold is commonly
achieved in an assay of 3040 cycles.
Products of the LCx assays are detected by a system
called microparticle enzyme immunoassay (MEIA). Each of a
pair of probes carries at its non-ligating end a molecule
(hapten) that is able to bind a specific antibody; the two
probes carry different haptens i.e. they bind different types of
antibody. Hence, after cycling, each ligated probe pair consists
of a copy of the target sequence flanked by two different
haptens (haptens 1 and 2). Microparticles (<1 m diam.), coated
with hapten 1-specific antibodies, are added to the system;
the microparticles bind hapten 1 on both ligated and nonligated probes. The microparticles are then immobilized on a
matrix. The non-ligated probes bearing hapten 2 are removed
by washing. A conjugate, consisting of alkaline phosphatase
covalently linked to a hapten 2-specific antibody, is then added
to the bound microparticles; the conjugate binds to hapten 2
(via the antibody), thus labelling ligated probe pairs (on the
microparticle) with alkaline phosphatase. A substrate for the
enzyme, 4-methylumbelliferyl phosphate, is then added and is
cleaved to the fluorescent product 4-methylumbelliferone; under
ultraviolet radiation, the rate at which fluorescence is generated
is proportional to the number of (enzyme-labelled) ligated probe
pairs. Readings above a certain cut-off value indicate a positive
result, i.e. evidence of a given sequence in the sample; readings
LD50
be extracted by cyanidation in the usual way. The ore is
crushed and subjected to bacterial action in highly aerated
bio-oxidation tanks; arsenopyrite (FeAsS) is solubilized by
oxidation (to FeAsO4 and sulphuric acid), thus exposing the
gold for cyanidation. After cyanidation, gold is separated from
the goldcyanide complex e.g. by adsorption to charcoal, and
the spent, cyanide-containing liquor is detoxified by bacteria;
detoxification involves the oxidation of cyanide to carbon
dioxide and urea, and the oxidation of urea to nitrate.
In addition to their use in leaching, bacteria have also been
used as bioadsorbents for the recovery of low levels of uranium
in certain liquid wastes.
(See also THIOBACILLUS.)
[Microbiology of metal leaching (symposium report): FEMS
Reviews (1993) 11 1267. Mining with microbes (review):
Biotechnology (1995) 13 773778. Predominant types of bacteria used in commercial bioleaching processes: Microbiology
(1999) 145 513.]
leader (leader sequence) A region of an RNA molecule (e.g.
certain mRNA molecules, pre-rRNA) between the 5 (promoter)
end and the sequence corresponding to the first (or only)
structural gene. The leader sequence is commonly non-coding,
but may encode a small regulatory peptide (a leader peptide):
see OPERON (attenuator control) and TNA OPERON.
leader peptidase See SIGNAL HYPOTHESIS.
leader peptide (1) See LEADER. (2) See SIGNAL HYPOTHESIS.
leading strand See DNA REPLICATION.
leaf blotch (scald) A CEREAL DISEASE, caused by Rhynchosporium secalis, which can affect e.g. barley and rye; large, pale
brown lesions with dark brown or purple margins appear mainly
on leaves, and crop losses may be severe. (See also FLUTRIAFOL
and PROPICONAZOLE.)
leaf curl (of peach) See TAPHRINA.
leaf nodules See PHYLLOBACTERIUM.
leafhopper A virus (LAV) An unclassified reovirus-like virus
which was isolated from the leafhopper Cicadulina bimaculata
during the search for the causal agent of MAIZE WALLABY EAR
DISEASE; attempts to infect maize plants with LAV have been
unsuccessful, and any connection between LAV and MWED
has yet to be proved. Although LAV resembles viruses of the
genus FIJIVIRUS, it cannot be included in the genus since it is not
known to infect any plant species.
leaky mutation A MUTATION which results in only partial inactivation of the sequence in which it occurs. (cf. NULL MUTATION.)
leather spoilage Leather has a relatively low pH (usually ca.
34) and even at high humidities is fairly resistant to bacterial
attack; however, at relative humidities of >80% leather is highly
susceptible to attack by moulds which may cause significant loss
of tensile strength. Aspergillus spp are commonly implicated,
but other moulds (e.g. species of Mucor, Paecilomyces and
Rhizopus) may also be involved. Heavy fungal contamination
may raise the pH sufficiently to allow some bacterial growth;
e.g. Bacillus sphaericus has been isolated from mouldy leather.
Preservatives which have been used for treating leather include
phenylmercuric salts of fatty acids, p-nitrophenol, and bnaphthol. (For the bating of hides by microbial enzymes see
PROTEASES.)
leben A type of concentrated YOGHURT consumed in e.g. Egypt.
Milk is fermented with organisms which include Lactococcus
lactis, Streptococcus thermophilus, Lactobacillus bulgaricus and
certain lactose-fermenting yeasts. The curd is concentrated by
draining off the whey and may then be dried. (See also DAIRY
PRODUCTS.)
Legionellaceae
phosphate group of phosphatidic acid is esterified with choline:
(CH3 )3 N+ (CH2 )2 OH.
lecithinase A PHOSPHOLIPASE (q.v.) which cleaves LECITHIN.
Extracellular lecithinases are formed e.g. by Bacillus cereus,
Clostridium bifermentans, C. novyi (g-toxin), C. perfringens (atoxin), and strains of Staphylococcus aureus; the lecithinase
of C. perfringens apparently requires Zn2+ for activity. Those
organisms (e.g. C. novyi, C. perfringens) which form lecithinases that are C-type phospholipases produce zones of opacity
around colonies when grown on e.g. EGG-YOLK AGAR due to the
formation of insoluble, phosphate-free diacylglycerides (diglycerides). (See also MILK SPOILAGE.)
lecithovitellin agar Syn. EGG-YOLK AGAR.
lectin pathway See COMPLEMENT FIXATION (c).
lectins Various non-enzymic proteins (usually glycoproteins)
which are not products of the immune system (thus excluding
antibodies) and which can each bind to specific carbohydrate
group(s) and can agglutinate (or precipitate) cells or other entities having these particular (and accessible) group(s). The term
lectin originally referred to certain plant products which bind
to and agglutinate particular types of erythrocyte (cf. PHYTOHAEMAGGLUTININ sense 2); it is now used for materials of plant,
animal or microbial origin which have specific carbohydratebinding ability though not necessarily in relation to erythrocytes. Lectins have been obtained e.g. from plants [Book ref. 37,
pp. 537547; ARPphys. (1985) 36 209234], lichens [Lichenol.
(1983) 15 303305], the snail (Helix pomatia), the horseshoe
crab (Limulus polyphemus), slime moulds (e.g. discoidins from
Dictyostelium discoideum, pallidins from Polysphondylium pallidum), fungi and bacteria (e.g. mannose-sensitive FIMBRIAE).
Lectins have been used e.g. for haemagglutination in blood
grouping studies. Many lectins behave as MITOGENS and are
used e.g. for lymphocyte activation in immunological studies.
In nature, lectins may be involved in plantmicrobe symbioses
[Book ref. 38, pp. 658677]; they may play a role in the
pathogenesis of some plant diseases [ARPpath. (1983) 21
300302] and possibly in certain animal diseases (e.g. lectins in
raw beans may promote disease in pigs by enhancing attachment
of ETEC to the ileal epithelium [CRM (1981) 8 303338 (324)]).
(See also GIARDIASIS.) [Interaction of bacteria and fungi with
lectins: ARM (1981) 35 85112.] (See also CONCANAVALIN A;
LIMULIN; PHYTOHAEMAGGLUTININ; POKEWEED MITOGEN; TRIFOLIIN
A; WHEAT GERM AGGLUTININ.)
lectotype A specimen, chosen to serve as NOMENCLATURAL TYPE,
derived from the original material studied by an author who did
not specify a HOLOTYPE; it has nomenclatural precedence over a
NEOTYPE.
LEE See PATHOGENICITY ISLAND.
leek yellow stripe virus See POTYVIRUSES.
left-handed DNA See e.g. Z-DNA.
left splice site See SPLIT GENE.
leghaemoglobin (leghemoglobin) A red haem-containing pigment present (in multiple forms) in the host cell cytoplasm
in the ROOT NODULES of leguminous plants. The protein and
haem moieties are specified by plant genes and bacteroid genes,
respectively. Leghaemoglobins are structurally and functionally
similar to animal myoglobins and haemoglobins but have a much
higher affinity for oxygen; they release bound oxygen only at low
levels of oxygen and thus permit aerobic respiration in the bacteroids while protecting NITROGENASE from oxygen inactivation.
[Book ref. 55, pp. 7379; ARPphys. (1984) 35 443478.]
Legionella See LEGIONELLACEAE.
Legionellaceae A family of Gram-negative, asporogenous
bacteria. Cells: rod-shaped or filamentous, 2.0 to >20.0
legionellosis
0.30.9 m; motile, with one, two or more polar or lateral
flagella. Cellular fatty acids are predominantly branched.
Aerobic; oxidase ve or weakly +ve. Chemoorganotrophic,
using amino acids (non-fermentatively) as carbon and energy
sources; carbohydrates are generally not metabolized. Growth
requires L-cysteine and iron (Fe3+ ) salts, and can occur
e.g. on blood agar supplemented with L-cysteine and iron,
on MuellerHinton agar supplemented with haemoglobin and
IsoVitaleX, or on buffered charcoalyeast extract agar (BCYE),
but not e.g. on unsupplemented blood agar or nutrient agar.
Optimum growth temperature: 3537 C. Gelatinase +ve;
catalase +ve; urease ve; NO3 not reduced. Several species
exhibit a bluish-white autofluorescence under WOODS LAMP, and
most species produce a diffusible brown pigment on tyrosinecontaining media. Species occur in various aquatic habitats: e.g.
surface waters, moist soils, thermally polluted streams, domestic
water systems, etc; most or all species can be pathogenic for man
(see LEGIONELLOSIS). GC%: ca. 3943; type genus: Legionella.
According to some authors [Book ref. 22, pp. 279288],
Legionella (type species L. pneumophila) is the sole genus
of the Legionellaceae, but other authors have divided the
family into three genera: Fluoribacter, Legionella and Tatlockia [IJSB (1980) 30 609614; IJSB (1981) 31 111115].
Species include e.g. L. bozemanii (Fluoribacter bozemanae;
WIGA bacterium), L. dumoffii (F. dumoffii ; Tex-KL bacterium), L. feeleii [AIM (1984) 100 333338], L. gormanii
(F. gormanii ), L. jordanis, L. longbeachae, L. micdadei (Tatlockia micdadei; TATLOCK agent; guinea-pig agent;
Pittsburg pneumonia agent), L. oakridgensis, L. pneumophila,
L. sainthelensi (AEM (1984) 47 369373], L. wadsworthii ).
[Taxonomy and typing of legionellae: RMM (1994) 5 7990.]
Sequencing of the mip gene has been reported to provide a
basis for unambiguous identification of 39 species of the genus
Legionella [Mol. Microbiol. (1997) 25 11491158; JCM (1998)
36 15601567.]
legionellosis Any (human) disease caused by a species of
Legionella (see LEGIONELLACEAE). Most species appear to be
capable of causing PNEUMONIA in man. Legionnaires disease is
a pneumonia caused by L. pneumophila. Infection is believed to
occur by inhalation of contaminated aerosols (common sources
of infection are air-conditioning cooling towers, showers, nebulizers, etc). [Survival of L. pneumophila in a model hot water
distribution system: JGM (1984) 130 17511756; distribution
and persistence of Legionella in water systems: MS (1985)
2 4043.] Incubation period: 210 days. Symptoms: malaise,
myalgia, headache, followed by fever, chills, and a consolidating pneumonia which primarily involves the alveoli and
terminal bronchioles; an intra-alveolar exudate is characteristic of the disease. Other common symptoms include chest
and abdominal pains, vomiting, diarrhoea, and mental confusion. Mortality rates may be high, particularly in compromised
individuals. [Review: Chest (1984) 85 114120.] An important feature of pathogenesis is the ability of L. pneumophila to
invade alveolar macrophages, to inhibit phagosomelysosome
fusion, and to multiply within these cells; such activity may
be facilitated by expression of the pathogens icm (= dot)
genes (see PHAGOCYTOSIS (a)) because mutations in these genes
can give rise to modified virulence [TIM (1998) 6 253255].
Moreover, the results of in vitro studies have suggested that
the pathogens zinc metalloprotease (a 38 kDa secreted protein; = tissue-destructive protease) may promote pathogenesis
by inhibiting both the oxidative burst and chemotaxis in phagocytic cells [JMM (2001) 50 517525].
Pontiac fever is an acute, febrile, non-pneumonic, selflimiting illness caused by L. pneumophila (and by L. feeleii
[AIM (1984) 100 333338]). Incubation period: ca. 36 hours.
Symptoms: fever, chills, headache, myalgia, arthralgia, diarrhoea, and sometimes neurological symptoms. Pittsburg pneumonia is a pneumonia caused by L. micdadei.
Lab. diagnosis: direct or indirect immunofluorescence tests
on e.g. sputum samples; microscopic examination of specimens
stained with e.g. DIETERLE SILVER STAIN; analysis of the fatty acids
of the isolated organism by GLC.
[Treatment: JAC (1999) 43 747752.]
Legionnaires disease See LEGIONELLOSIS.
legume bloat See BLOAT.
legume yellows virus See LUTEOVIRUSES.
leguminous root nodules See ROOT NODULES.
Leidenfrost phenomenon
The formation of a heat-insulating
layer of gaseous nitrogen around a specimen when it is plunged
into liquid nitrogen. (See also FREEZING.)
Leifsons flagella stain (for bacterial flagella) Mix equal volumes of 1.5% w/v aqueous NaCl and 3% w/v aqueous tannic acid; to this mixture add half its volume of a solution of
pararosanilin acetate (0.9% w/v) and pararosanilin hydrochloride (0.3% w/v) in 95% ethanol. Prepare a medium-free, slightly
cloudy suspension of bacteria in distilled water. Using a wax
pencil, draw a ring on a chemically clean glass slide enclosing
ca. 2 cm2 . Spread one loopful of the bacterial suspension within
the ringed area; dry at room temperature. Do not fix. Add 1 ml
stain; allow to act for ca. 10 min and rinse off gently under the
tap. Flagella appear to be coated with a colloidal tannic aciddye
complex, rendering them visible by light microscopy.
Leighton tube A test-tube in which part of the wall (near
the closed end) forms a flat, rectangular region which can
accommodate a cover-glass on which a cell monolayer can be
formed.
Leiotrocha See PERITRICHIA.
LeishmanDonovan bodies Amastigote forms of Leishmania in
the vertebrate host.
Leishmania A genus of parasitic protozoa (family TRYPANOSOMATIDAE) which resemble TRYPANOSOMA species in their ultrastructure. The organisms are the causal agents of LEISHMANIASIS
in mammals, and are transmitted by sandflies of several genera
(e.g. Lutzomyia, Phlebotomus, Sergentomyia); species of Leishmania which are normally dermatotropic sometimes give rise
to visceral leishmaniasis, while typically visceralizing strains
sometimes cause cutaneous infections. Most leishmaniases are
zoonotic.
In the vertebrate host Leishmania grows in the intracellular,
amastigote form (ca. 210 m in diam.) primarily in mononuclear phagocytes (e.g. macrophages). (Leishmania species can
grow within phagolysosomes: see PHAGOCYTOSIS; amastigote
forms of L. donovani have been found to contain CATALASE and
glutathione peroxidase in amounts greater than those found in
the promastigote stage. The ability of Leishmania spp to undergo
ANTIGENIC VARIATION may contribute to their pathogenicity.)
In the sandfly the pathogen occurs in the paramastigote and
promastigote forms, the latter being the form infective for man.
In cell-free media (e.g. in NNN MEDIUM), and in tissue culture,
the organisms grow in the promastigote form.
Leishmania spp include L. aethiopica, L. braziliensis, L. donovani, L. major, L. mexicana and L. tropica. Some species are
divided into subspecies; e.g., L. braziliensis includes e.g. L.
braziliensis braziliensis (= L. b. braziliensis), L. b. guyanensis
and L. b. peruviana. Organisms which cause visceral leishmaniasis have been given separate names in particular geographical
432
lepromin test
regions: e.g. L. infantum (Mediterranean), L. chagasi (S. America), and L. archibaldi (Sudan); some authors regard all of these
as one species, L. donovani [Book ref. 72, p. 215].
Leishmania spp have been divided into groups (sections)
on the basis of their location within the arthropod vector:
see HYPOPYLARIA, PERIPYLARIA, SUPRAPYLARIA; at least some of
the reptile-infecting species in the Hypopylaria and Peripylaria
appear to be trypanosomes (L. tarentolae has been renamed
Trypanosoma platydactyli ).
leishmanial form Obsolete Syn. AMASTIGOTE.
leishmaniasis Any disease caused by a species of LEISHMANIA;
see CUTANEOUS LEISHMANIASIS, MUCOCUTANEOUS LEISHMANIASIS,
POST-KALA-AZAR DERMAL LEISHMANIASIS and VISCERAL LEISHMANIASIS. [Book ref. 72, pp. 183249.]
leishmaniasis recidivans An intractable form of CUTANEOUS
LEISHMANIASIS which may develop after an apparent cure of a
previous episode of cutaneous leishmaniasis; lesions, typically
non-ulcerating, form around the rim of scar tissue.
leishmanin test Syn. MONTENEGRO TEST.
Leishmans stain See ROMANOWSKY STAINS.
Leloir pathway See LACTOSE and Appendix III(a).
Lelystad virus See BLUE-EARED PIG DISEASE.
Lemanea See RHODOPHYTA.
Leminorella A new genus of non-motile Gram-negative bacteria
of the ENTEROBACTERIACEAE; two species have been described:
L. grimontii (the proposed type species) and L. richardii [JCM
(1985) 21 234239]. Reactions: e.g. VP ve; indole ve; H2 S
+ve; LDC ve; ODC ve; ADH ve; no growth with KCN.
Species are relatively inactive biochemically; acid is produced
from L-arabinose and D-xylose, but not from a wide range of
other sugars (including lactose). Strains have been isolated from
human faeces and urine.
Lempholemma
A genus of gelatinous LICHENS (order
LECANORALES); photobiont: Nostoc. Thallus: homoiomerous,
lacking a cortex. HORMOCYSTS are formed in specialized swollen
regions of the thallus (termed hormocystangia), and hyphae of
the mycobiont are or may be associated with the gelatinous
sheath of the hormocyst.
lens-shaped A phrase sometimes used to describe the shape
of a structure or colony etc; as a descriptive phrase it is of
doubtful value since a lens may be double-convex, plano-convex,
meniscus etc. (cf. LENTICULAR.)
lentic Pertaining to aquatic habitats with standing (still) water
(e.g. ponds, swamps). (cf. LOTIC.)
lenticular (lentiform) Shaped like a lentil or a double-convex
lens.
lentiform Syn. LENTICULAR.
Lentinula
A genus of fungi of the family Tricholomataceae (order AGARICALES). L. edodes (formerly Lentinus edodes) forms edible fruiting bodies: see SHII-TAKE. [Chemically
defined medium for the fruiting of L. edodes: Mycol. (1983)
75 905908; note on the reclassification of Lentinus edodes to
Lentinula edodes: MS (1986) 3 171; effect of light and aeration
on fruiting of L. edodes: TBMS (1987) 88 920.] (See also
MYCOVIRUS.)
Lentinus A genus of lignicolous fungi of the APHYLLOPHORALES
(family Polyporaceae) which form tough but pliant basidiocarps
in which the hymenium is borne on lamellae (see LAMELLA).
L. lepideus forms a mushroom-shaped basidiocarp in which
the fawn-coloured pileus bears dark scales and is supported
by a central or eccentric stipe; the lamellae are whitish and
decurrent, and the basidiospores are ellipsoidal, hyaline, and
ca. 10 5 m. L. lepideus causes TIMBER SPOILAGE (see also
433
leprose
Laboratory diagnosis. Biopsies from skin lesions, or e.g. nasal
secretions, are stained by acid-fast stains; in lepromatous leprosy
the foamy Virchow cells, packed with acid-fast bacilli, are
diagnostic. Tuberculoid leprosy may be difficult to differentiate
from sarcoidosis or non-leprosy mycobacterial granulomas.
(See also LEPROMIN TEST.) The carbohydrate moiety of PGLI (an M. leprae cell-surface glycolipid) may be useful in a
serodiagnostic test.
Chemotherapy. Currently, antimicrobial treatment involves a
combination of drugs: DAPSONE and rifampicin with or without
CLOFAZIMINE. Other drugs (e.g. ofloxacin, minocycline) are also
effective for treating leprosy. Thalidomide is useful in some
cases of ENL.
[Various aspects: TRSTMH (1993) 87 499517; epidemiology: FEMS (1996) 136 221230; review: RMM (1998) 9
3948.]
lepto- Prefix meaning fine, narrow, thin.
Leptogium A genus of gelatinous LICHENS (order LECANORALES);
photobiont: Nostoc. The thallus has a cortex, but otherwise
resembles that of COLLEMA spp (although generally less gelatinous and often felt-like or tomentose). [Studies on some species:
Lichenol. (1983) 15 109125.]
Leptolegnia See SAPROLEGNIALES.
Leptomitales An order of aquatic fungi (class OOMYCETES) which
are typically saprotrophic though one species, Leptomitus
lacteus, may be an opportunist invader of epidermal lesions in
fish. The thallus consists of hyphae which bear characteristic
constrictions along their lengths, the constrictions often being
plugged with CELLULIN GRANULES; in some genera (Apodachlya,
Leptomitus) there is evidence that the cell wall contains both
CHITIN and CELLULOSE [Book ref. 174, pp. 6263]. Other genera
include Aqualinderella (an anaerobe found in polluted waters)
and Rhipidium.
Leptomitus See LEPTOMITALES.
leptomonad form Obsolete syn. PROMASTIGOTE.
Leptomonas A genus of homoxenous parasitic protozoa (family
TRYPANOSOMATIDAE) which typically occur in the gut (sometimes
in the haemocoele or in the salivary glands) of insects. The
organisms occur in amastigote and promastigote forms, the latter
usually being 1040 m in length (excluding flagellum), or
about twice as long including the flagellum; in some species
the cell may be helical, up to 200 m in length.
leptomycin B A product of SECONDARY METABOLISM (in Streptomyces spp) which blocks progression through the cell cycle in
eukaryotic cells.
Leptomyxa See ACARPOMYXEA.
Leptonema A genus of bacteria of the order SPIROCHAETALES.
[Motility in L. illini : see e.g. JB (1996) 178 65396545.]
Leptosphaeria
A genus of fungi (order DOTHIDEALES) which
include saprotrophs and plant parasites (see e.g. BLACKLEG
(sense 2), CANE BLIGHT and GLUME BLOTCH); anamorphs occur
in e.g. Camarosporium and Septoria.
Leptospira
A genus of obligately aerobic bacteria (family
LEPTOSPIRACEAE) which occur as free-living organisms in soil
and aquatic (freshwater and marine) habitats, and as parasites
or pathogens in man and other animals (see LEPTOSPIROSIS). The
cells are motile, helical (18 coils/cell), 0.1 m in diameter and
from 6 to over 12 m in length; a single periplasmic flagellum
arises at each end of the cell. In liquid media, one or both
ends of the cell are typically bent or hooked. Growth occurs
on e.g. serum-containing media; optimum growth temperature:
2830 C. Metabolism is respiratory (oxidative); fatty acids are
metabolized by b-oxidation to acetate and CO2 . Catalase and/or
Leuconostoc
peroxidase +ve; oxidase +ve. GC%: 3541, but one strain 53.
Type species: L. interrogans.
Two species are recognized [Book ref. 22, pp. 6267]:
L. biflexa (free living, capable of growth at 13 C, usually
resistant to 225 g/ml 8-azaguanine) and L. interrogans (parasitic/pathogenic, usually sensitive to 225 g/ml 8-azaguanine,
and growth inhibited at 13 C). Each species consists of a
large number of named serotypes (= serovars) which are classified into named serogroups; thus, e.g. the Icterohaemorrhagiae
serogroup of L. interrogans contains nearly twenty serotypes,
including e.g. dakota and icterohaemorrhagiae.
Leptospiraceae A family of aerobic bacteria of the order
SPIROCHAETALES; the cells typically have hooked ends, their cell
wall PEPTIDOGLYCAN contains the diamino acid diaminopimelic
acid, and their carbon and energy sources are long-chain fatty
acids or long-chain fatty alcohols (cf. SPIROCHAETACEAE). One
genus: LEPTOSPIRA.
Leptospirillum ferrooxidans See LEACHING.
leptospirosis A disease of man and animals, caused by any of
various serotypes of Leptospira interrogans. A wide range of
animals can act as carriers, the leptospires normally occurring in
the kidney tubules; e.g., serotypes icterohaemorrhagiae and australis A are carried by rats and other rodents, canicola by dogs
and pigs, pomona by cattle and pigs, hardjo and grippotyphosa
by cattle. In domestic animals the disease ranges from mild to
fatal, depending on the animal and serotype involved; symptoms
commonly include fever, jaundice, haematuria (cf. RED WATER),
and abortion. (Rodents appear not to be significantly affected
by leptospire infection.) Animals may continue to excrete leptospires in their urine for several months after recovery.
Man acquires infection either by direct contact with animals
or animal carcasses (cf. ZOONOSIS) or via water contaminated
with urine from infected animals. Infection occurs via wounds
or mucous membranes. Incubation period averages ca. 10
days. In the mild form of leptospirosis, onset is abrupt with
shivering, fever, prostration, headache, anorexia and myalgia;
nausea and vomiting may occur. Renal function is typically
impaired, with proteinuria, haematuria etc. Uveitis is a late
complication. A severe form of leptospirosis (Weils disease,
infectious jaundice) is caused by serotype icterohaemorrhagiae;
symptoms are more intense, with e.g. marked prostration,
severe nausea, vomiting and diarrhoea, enlargement of the
liver, jaundice, renal dysfunction, haemorrhages, MENINGITIS.
Mortality rates: ca. 1540%. Lab. diagnosis: demonstration of
rising titres of antibodies (which appear 710 days after onset);
identification/culture of the pathogen from blood during the first
week, later from urine. [ELISA for detection of specific IgM
and IgG in human leptospirosis: JGM (1985) 131 377385.]
leptotene stage See MEIOSIS.
Leptotheca See MYXOSPOREA.
Leptothrix
A genus of Gram-negative IRON BACTERIA. Cells:
polarly flagellated single rods, or chains of rods within a sheath.
Type species: L. ochracea.
Leptotrichia
A genus of Gram type-negative bacteria (family BACTEROIDACEAE) which occur e.g. in the human mouth.
Cells: non-motile, straight or slightly curved rods, 0.81.5
5.015.0 m, often occurring in pairs, chains or septate filaments; the cells of young cultures may stain Gram-positively,
but the cell wall resembles those of Gram-negative bacteria.
Acid (no gas) is formed from carbohydrates; glucose fermentation yields lactic acid with small amounts of acetic and succinic
acids. GC%: ca. 25. Type species: L. buccalis.
lesion A localized region of tissue which has been damaged
physically or altered by any pathological process.
Leucopaxillus
as a result of immunological or non-immunological stimuli;
leukotrienes can e.g. cause contraction of smooth muscle, stimulate vascular permeability, and act as attractants for leucocytes.
[Review: ARB (1983) 52 355377.]
leukoviruses Former name for retroviruses of the ONCOVIRINAE,
particularly the TYPE C ONCOVIRUS GROUP.
levamisole A drug used to stimulate the immune response;
inhibit tumour formation; stimulate the phagocytic activity
of macrophages; inhibit alkaline phosphatases; treat intestinal
disease caused by certain helminths e.g. that caused by Ascaris
lumbricoides.
levan A linear FRUCTAN consisting mainly of (2 6)-b-linked
fructofuranose residues. Levans are widespread as storage
polysaccharides in higher plants (especially grasses), and are
produced as extracellular slime by certain bacteria (e.g. species
of Bacillus and Streptococcus). (See also ROPINESS and DENTAL
PLAQUE.)
Leveillula See ERYSIPHALES.
Levinea See CITROBACTER.
Levinthals medium A medium used for the isolation of
Haemophilus spp; it contains both V FACTOR and X FACTOR.
Levinthal stock is made by adding defibrinated horse blood
(10%) to a boiling brainheart infusion broth and filtering
through e.g. glass wool and then through a membrane filter.
Autoclaved peptone broth is then added, and the whole may be
mixed with sterile molten agar and dispensed into Petri dishes.
[Recipe: Book ref. 46, pp. 13751376.]
Leviviridae A family of BACTERIOPHAGES [Book ref. 23, p. 136];
the genome is linear, positive-sense ssRNA (MWt ca. 1.01.3
106 ), and the virion is icosahedral (ca. 2226 nm diam.). One
genus: Levivirus.
Leviviruses occur e.g. in enterobacteria (e.g. phages a15, b,
f2, fr, M12, MS2, 2, Qb, R17 and R23), in Pseudomonas (e.g.
PP7, 7S) and in Caulobacter.
Enterobacterial leviviruses (common in sewage) have been
classified into four groups (IIV) on the basis of serological and
physiological properties. Phages of group I (e.g. f2, fr, MS2,
R17) and group III (e.g. Qb) have been the most intensively
studied. (MS2, f2 and R17 apparently differ only in a number
of point mutations.)
The group I virion consists of (i) 180 copies of a single type
of coat protein, (ii) one molecule of A protein (= maturation
protein necessary for infectivity and phage maturation), (iii)
the RNA genome, and (iv) at least in MS2, spermidine (presumably to neutralize the negative charge on RNA). (The Qb virion
is similar but contains one molecule of an A2 protein (equivalent to A protein in group I phages) and about three molecules
of an A1 protein (= IIb protein); the A1 protein is formed by
READTHROUGH of the coat protein gene.) [Capsomeric structure
of Qb: Nature (1982) 298 819824.]
The group I phage genome encodes: (i) the A protein; (ii) the
coat protein; (iii) a replicase subunit; and (iv) a lysis protein
(the gene for which overlaps the coat and replicase genes in the
+1 reading frame [Nature (1982) 295 3541]). The lysis protein
(L protein) of MS2 forms specific adhesion sites (junctions of
the cytoplasmic and outer membranes); these sites may facilitate
lysis of the cell envelope [JB (1989) 171 33313336].
In Qb and other leviviruses the replicase subunit combines
with three host proteins the S1 protein of the 30S ribosomal subunit, and the elongation factors EF-Tu and EF-Ts (see
PROTEIN SYNTHESIS) to form the active replicase (i.e. RNAdependent RNA polymerase) necessary for phage genome replication. Expression of viral genes is controlled in both quantity
lichen
and time; thus, e.g. coat protein is synthesized greatly in excess
of A protein, and it acts as a repressor which, later in infection,
terminates translation of the replicase subunit gene. Regulation
of gene expression may involve changes in the secondary structure of the RNA which alter the availability of ribosome binding
sites [e.g. Nature (1982) 295 3541]. Virion assembly apparently occurs largely or exclusively by spontaneous aggregation.
Most or all enterobacterial leviviruses are male-specific
(ANDROPHAGES); f2, MS2, R17, fr, M12 and Qb all adsorb specifically to the sides of F pili (cf. INOVIRUS). The Pseudomonas
phages PP7 and 7S adsorb to the chromosomally specified polar
(PSA) fimbriae. Caulobacter phages also adsorb to polar fimbriae; only the pre-divisional and swarmer stages are susceptible
to infection. Infection of the host cell may, at least in some cases,
involve pilus (or fimbria) retraction. The genome enters the host
cell together with and probably mediated by the A/A2 protein (which is cleaved during penetration).
Levivirus See LEVIVIRIDAE.
levofloxacin A QUINOLONE ANTIBIOTIC (q.v.).
levulose D-Fructose.
lexA gene See SOS SYSTEM.
LFA-1 See INTEGRINS.
LFA-2 See IMMUNOGLOBULIN SUPERFAMILY.
LFA-3 See IMMUNOGLOBULIN SUPERFAMILY.
LFT (of plasmids) See EPIDEMIC SPREAD.
LFT lysate See TRANSDUCTION.
LGLs Large granular lymphocytes: see NK CELLS.
LHC LIGHT-HARVESTING COMPLEX.
LHC complex See CELLULOSE.
library (gene bank; gene library) (mol. biol.) A collection of
recombinant DNA molecules which, together, commonly represents the entire genome of an organism (a genomic library)
(see figure).
Another type of library consists of a collection of CDNA
molecules derived from a mixture of polyadenylated mRNAs
isolated from a population of cells of a given strain; this kind of
library does not represent the entire genome of the strain.
Licea See MYXOMYCETES.
Liceales See MYXOMYCETES.
lichen A composite organism consisting of a fungus (the mycobiont) and an alga or cyanobacterium (the photobiont cf. PHYCOBIONT) in symbiotic association; a lichen thallus is morphologically and physiologically quite unlike that of either symbiont
growing separately. Lichens are widely distributed, being found
from tropical to polar regions in a very wide range of habitats, both terrestrial (e.g. on trees, rocks and soil) and aquatic
(freshwater and marine).
Taxonomically, lichens are generally regarded as lichenized
fungi, classification being based mainly on the nature and origin of their fruiting structures. Most mycobionts appear not to
occur in free-living form (but cf. XANTHORIA). The majority
are ascomycetes (ascolichens) belonging mainly to the orders
ARTHONIALES, CALICIALES, DOTHIDEALES, GRAPHIDALES, GYALECTALES, LECANIDIALES, LECANORALES, OPEGRAPHALES, PELTIGERALES, PERTUSARIALES, PYRENULALES, TELOSCHISTALES, and VERRUCARIALES. Some lichens belong to the Deuteromycotina, and
a few to the Hymenomycetes (basidiolichens).
The photobiont is usually either a green alga (e.g. Coccomyxa, Myrmecia, Phycopeltis, Pseudotrebouxia, Trebouxia
or Trentepohlia) or a cyanobacterium (usually Nostoc or
Calothrix ). Some lichens may have more than one photobiont:
see e.g. SOLORINA and CEPHALODIUM. Free-living counterparts of
lichen photobionts occur in nature, but in the lichen the cells
DNA ligase
437
lichen
Vitamins found to be necessary for the growth of the
mycobiont in culture are assumed to be supplied by the
photobiont in nature.
Lichens accumulate high concentrations of certain metal ions
(including heavy metals), but lichen mineral metabolism is not
well understood.
Water (in liquid or vapour form) is readily absorbed by lichen
thalli; the absorbed water occurs intercellularly and is readily
lost by evaporation. The ability to absorb and retain water may
be influenced by thallus morphology e.g., surface area and
hence absorptive capacity will be greater in a thallus which is
extensively lobed or perforated than in one which is not. (See
also RHIZINE.)
Lichen substances (lichen acids). Lichen mycobionts produce a range of water-insoluble secondary metabolites (e.g.
higher aliphatic acids and esters, depsides, depsidones, dibenzofurans, anthraquinones) which may be deposited on the
medullary hyphae, on the surface of the cortex (often giving a pruinose appearance), in the hymenial discs (see e.g.
RHODOCLADONIC ACID), etc. Many of these substances are unique
to lichens; they are generally not formed by the isolated mycobionts. Their functions are largely unknown, but may include
e.g. protection of the photobiont from high light intensities (see
e.g. PARIETIN); inhibition of potentially competing plants (particularly bryophytes) and/or soil microflora in the vicinity of the
thallus (e.g. EVERNIC ACID and USNIC ACIDS have antibiotic activity); prevention of grazing of the thallus by invertebrates; etc.
The content of lichen substances in a given lichen is a useful feature in taxonomy and identification. The compounds may
be identified e.g. by chromatography, mass spectrometry, microcrystallography etc. Some lichen substances give characteristic
colour reactions with certain reagents, and this forms the basis
of simple colour tests widely used for identification of lichens
in the field. The reagents used are: saturated aqueous calcium
hypochlorite (C), 1025% aqueous KOH (K), and 15%
ethanolic p-phenylenediamine (P or PD). For example, parietin and other anthraquinones give a purple colour with K.
Growth of a lichen thallus generally appears to occur at or near
the periphery (or apex in fruticose thalli). [Growth in circular
thalli: Lichenol. (1981) 13 265287.] Lichen growth is characteristically slow; the radius of a circular thallus may increase
by (e.g.) 0.012.50 mm per year, depending on species, rainfall, light intensity, temperature, etc. (See also LICHENOMETRY.)
In certain crustose and squamulose lichens (e.g. Pannaria, Pertusaria, Rhizocarpon) a photobiont-free margin (the hypothallus)
may be formed around the thallus as the hyphae of the mycobiont grow outwards; the photobiont reproduces by cell division
or e.g. by autospore formation, and the daughter cells spread
into the region of new fungal growth.
Reproduction. Asexual (vegetative) reproduction in lichens
may be achieved e.g. by SOREDIUM, ISIDIUM or HORMOCYST
formation, or by fragmentation of the thallus. Some lichens may
be able to generate new thalli from conidia (which may or may
not be produced in pycnidia, according to species).
Sexual reproduction commonly involves ascocarp formation.
Lichen ascocarps tend to be longer-lived than those of nonlichenized ascomycetes, and may continue to produce ascospores
for a period of years. Since ascospores do not contain the photobiont, the germinating ascospores must acquire the photobiont
from the environment. In a few cases (e.g. Endocarpon sp,
Pertusaria pertusa) cells of the photobiont may adhere to the
ascospores as they are released, thereby allowing their dissemination with the ascospores. In most cases, however, the fungus
light chain
regions which were subjected to fall-out from atmospheric
nuclear weapons tests in the 1950s/1960s; lichens in this region
form the basis of the food chain: lichen reindeer (caribou)
man, and correspondingly high levels of e.g. 137 Cs were recorded
in Lapps who consumed reindeer meat at that time (although the
levels were not considered to be dangerous).
[Lists of references on lichens and air pollution are published
regularly in The Lichenologist.]
Uses of lichens. Some lichens are used as food by people
in certain countries: e.g. Cetraria islandica (Iceland moss) is
consumed e.g. in Iceland, Umbilicaria esculenta (iwatake) in
Japan. Species of Cladonia and Cetraria form a major part of
the winter diet of reindeer (caribou) and other deer in arctic
regions. Various lichens have been used since ancient times as
sources of dyes: e.g. Ochrolechia tartarea yields the purple
dye cudbear, Parmelia spp a brown dye, and Roccella spp
LITMUS and the purple dye orchil. Certain lichens particularly
Evernia prunastri (oakmoss) are used in the manufacture
of perfumes, both for their own scent and for their ability to
stabilize (fix) other scents. Lichens were formerly widely used
in folk medicine; currently, USNIC ACIDS have some medical
uses. In Scandinavian countries, Cladonia stellaris is harvested
on a commercial scale for ornamental uses in wreaths, floral
decorations etc [Lichenol. (1979) 11 8589].
lichen starch Syn. LICHENIN.
lichenan Syn. LICHENIN.
lichenicolous Growing on lichens.
lichenin (lichenan; lichen starch; moss starch) A linear b-Dglucan consisting mainly of (1 3)-b-linked cellotriose units
(i.e. units of three (1 4)-b-linked glucose residues); it occurs
in certain lichens (e.g. Cetraria islandica). (cf. ISOLICHENIN.)
lichenometry A method for dating glacial deposits, stone monuments etc, based on a knowledge of the growth rates of particular (usually crustose) lichens. The assumption is made that
the largest crustose thalli present on a given exposed surface
started to grow when the surface first became exposed; the thalli
are measured, and their ages estimated from a standard growth
curve for the species thus giving an approximate age for the
substratum. Certain thalli of Rhizocarpon geographicum have
been estimated to be ca. 10004500 years old. [Lichenometry
with R. geographicum: Lichenol. (1983) 15 249261.]
Lichina A genus of small, fruticose LICHENS (order LECANORALES);
photobiont: a cyanobacterium. The thallus is more or less gelatinous, brown to black, erect, branching, terete (L. confinis) or
flattened (L. pygmaea), forming tufts or mats on rocks on the
seashore at or just above the high-tide level. Apothecia occur
immersed in the swollen ends of the branches.
Lieberkuehnia See GRANULORETICULOSEA.
Lieberkuhns
organelle (watchglass organelle) A refractive, len
ticular body which occurs, subpellicularly, in or near the buccal
cavity in certain hymenostomes.
lif gene See LYSOSTAPHIN.
lig gene Gene for DNA LIGASE.
ligase chain reaction See LCR.
ligases (synthetases) ENZYMES (EC class 6) which catalyse covalent bond formation using energy obtained from the cleavage
of a pyrophosphate bond (e.g. in ATP); CO, CS, CN and
CC bonds are formed by different subclasses of ligases. (See
e.g. DNA LIGASE; cf. SYNTHASE.)
ligative hyphae See HYPHA.
light chain (immunol.) The smaller (MWt ca. 23000) of the two
types of polypeptide chain in an IMMUNOGLOBULIN monomer.
About half the (ca. 215) amino acid residues in a light chain
light green
units connected by CC and COC links; it is formed
by the peroxidase-initiated dehydrogenative polymerization of
substituted p-hydroxycinnamyl alcohols (p-coumaryl, coniferyl
and sinapyl alcohols). Lignin is a major component in the
vascular tissues of terrestrial plants, and constitutes ca. 2035%
of the weight of wood; it occurs with hemicelluloses in the
matrix of the cell walls, waterproofing the xylem vessels
and providing mechanical strength and protection from enzymic
attack. [Lignification in disease resistance in plants: ARPpath.
(1980) 18 259288.] Lignin is tightly bonded to CELLULOSE and
HEMICELLULOSES mainly by hydrogen bonds but also by some
covalent bonds.
Lignins are extremely resistant to chemical and enzymic
degradation; biological degradation is achieved mainly by
fungi most efficiently by white-rot basidiomycetes (see WHITE
ROT) but also by certain actinomycetes. In the white-rot fungi
Phanerochaete chrysosporium and Coriolus versicolor, lignin
degradation is a secondary metabolic process, occurring under
low levels of nutrient nitrogen and requiring the presence of
a carbon source such as glucose or cellulose [Book ref. 39,
pp. 6790]; it appears not to yield significant carbon or energy,
but allows access to the polysaccharide components of the cell
walls (see CELLULASES). P. chrysosporium produces an extracellular haemoprotein ligninase which, in the presence of H2 O2 ,
can degrade lignin by bringing about oxidative cleavage of
the backbone between Ca and Cb, oxidation and hydroxylation of benzylic methylene groups, oxidation of phenols and
benzyl alcohols, etc. The haemoprotein functions as a peroxidase. Reaction of the enzyme with H2 O2 generates a highredox-potential porphyrin cation radical (oxy-ferryl complex)
which can extract a single electron from an aromatic ring in
the lignin substrate to generate an aromatic cationic radical;
this is followed by a variety of spontaneous degradative reactions via radical and cation intermediates [FEBS (1985) 183
712, 1316]. P. chrysosporium produces multiple forms of
the haemoprotein lignin peroxidase [homology among multiple
extracellular peroxidases from P. chrysosporium: JBC (1987)
262 419424]. Other enzymes implicated in aerobic lignin
degradation include phenol oxidases (e.g. LACCASE) and alcohol
oxidase. Quinones, which can be toxic to organisms, are common products of phenol oxidase action; several white-rot fungi
produce a cellobiose:quinone oxidoreductase which couples the
oxidation of cellobiose with the reduction of quinones [Book
ref. 26, pp. 2526], thus linking cellulose and lignin degradation. [Anaerobic lignin degradation: AEM (1984) 47 9981004.]
ligninolytic Capable of degrading LIGNIN. (cf. LIGNOLYTIC.)
lignite biodegradation See COAL BIODEGRADATION.
lignocellulose A complex containing LIGNIN, CELLULOSE, and
(usually) HEMICELLULOSES.
lignolytic Capable of degrading wood. (cf. LIGNINOLYTIC.)
Limacella See AGARICALES (Amanitaceae).
limax amoebae Slug-like amoebae, i.e., cylindrical (not flattened) MONOPODIAL AMOEBAE, or cylindrical amoebae which flow
along without forming obvious pseudopodia.
limberneck A form of BOTULISM in birds, especially poultry,
caused by C. botulinum type A. (cf. WESTERN DUCK DISEASE.)
Limburger cheese See CHEESE-MAKING.
lime sulphur See SULPHUR.
limit dextrin See AMYLASES.
limit dextrinase See DEBRANCHING ENZYMES.
limit of resolution See RESOLVING POWER.
limited enrichment method See AUXOTROPH.
limulin A LECTIN from the horseshoe crab, Limulus polyphemus;
it is presumed to bind at sites in LIPOPOLYSACCHARIDES and
lipopolysaccharide
glycerol moiety. Lipases function well at the interface between
their hydrophobic substrates and the aqueous phase, and can act
on triglycerides in micelles or emulsions.
Microbial lipases have some commercial applications. They
are used e.g. in digestive aids, in the manufacture of certain
cheeses (to improve or accelerate the development of flavour
and aroma) and in INTERESTERIFICATION.
Tests for bacterial lipase production: (a) growth on EGG-YOLK
AGAR; (b) TWEEN HYDROLYSIS; (c) inoculation onto a nutrient agar
medium containing a fat (or e.g. corn oil) and NILE BLUE (lipaseproducing colonies have a blue halo). A given lipase may not
react positively in all tests. (See also FILM AND SPOTS.)
lipid A See LIPOPOLYSACCHARIDE.
lipid A-associated protein See ENDOTOXIN.
lipid cyst See METHYLOCOCCACEAE.
lipid stain See e.g. BURDONS STAIN.
lipid X See LIPOPOLYSACCHARIDE.
lipoamino acids See bacterial CYTOPLASMIC MEMBRANE.
lipofection Lipid-aided insertion of nucleic acid into mammalian
(and other) cells; uptake is promoted when (e.g.) DNA forms
LIPOSOMES with mixed cationic and neutral lipids.
lipoic acid (a-lipoic acid; thioctic acid) A coenzyme which is
involved in the oxidative decarboxylation of keto-acids: e.g.
pyruvate and 2-oxoglutarate are decarboxylated to acetyl-CoA
and succinyl-CoA, respectively [see Appendix II(a)]. (See also
THIAMINE.) The oxidized form of the coenzyme contains a
disulphide bond (SS) which can be reduced to form two
SH groups, the reduced coenzyme (dihydrolipoic acid) being
6,8-dithiooctanoic acid: CH2 SH.CH2 .CHSH.(CH2 )4 .COOH.
Lipoic acid is required as a growth factor e.g. by Tetrahymena spp; it can replace acetate as a growth factor for e.g.
Lactobacillus casei.
(See also ARSENIC.)
Lipomyces A genus of yeasts (family SACCHAROMYCETACEAE).
Cells are spherical or ovoid; vegetative reproduction occurs by
multilateral budding or by bud-fission. In most species the cells
are each surrounded by a thick mucoid capsule which often
contains a starch-like polysaccharide. Cells accumulate lipid,
and those from older cultures usually contain one or more
lipid globules. Asci typically develop from active buds; an
active bud resembles a vegetative bud but develops into an
ascus either following conjugation between the active bud
and a protuberance on another cell (or the same cell), or
in the absence of conjugation. The mother cell of the active
bud may also become an ascus. Ascospores are ellipsoidal or
oblong-ellipsoidal, light amber to brown, smooth, or e.g. rough
with longitudinal ridges, 220 or more per ascus (depending
on species). [Ascospore morphology and ultrastructure: IJSB
(1984) 34 8086.] The organisms are non-fermentative and
do not assimilate NO3 . Species (L. anomalus, L. kononenkoae,
L. lipofer, L. starkeyi, L. tetrasporus) have been isolated from
soil. [Book ref. 100, pp. 252262.]
lipo-oligosaccharide (LOS) In certain Gram-negative bacteria
(e.g. Neisseria meningitidis): a (normal) component of the OUTER
MEMBRANE which is anatomically equivalent to LIPOPOLYSACCHARIDE (q.v.) but in which the O-specific chains are shorter
than those (for example) in the enterobacteria [CRM (1998) 24
281334].
lipopolysaccharide (LPS) Strictly: any lipid-containing polysaccharide; however, the term lipopolysaccharide is commonly
used to refer specifically to the endotoxic component of the
OUTER MEMBRANE in Gram-negative bacteria. Outer membrane
LPS is a complex molecule consisting of three covalently linked
lipopolysaccharide-binding protein
(KDO-PEtN)
GlcNAc
O-specific chain
Glc
Gal
(Gal)
(Hep)
Glc
Hep
(PPEtN) (KDO)
Hep
KDO
Lipid A
P
LIPOPOLYSACCHARIDE. General structure of the core oligosaccharide in Salmonella typhimurium; the structure is somewhat variable, and possible sites of variation are indicated by parenthesis. Glc = D-glucose; Gal = D-galactose; Hep = heptose (L-glycero-D-mannoheptose); KDO =
3-deoxy-D-manno-octulosonate; GlcNAc = N-acetyl-D-glucosamine; PEtN = phosphorylethanolamine; PPEtN = pyrophosphorylethanolamine; P = phosphate. [Data from e.g. Book ref. 138, pp. 157207.]
listeriosis
liposarcoma See SARCOMA.
liposome An artificial phospholipid vesicle. Liposomes have
many uses in biology. For example, various components of biological membranes (e.g. PORINS, viral ENVELOPE proteins) can
be incorporated into liposomes, allowing investigation of their
properties under controlled conditions. Enzymes can be immobilized (see IMMOBILIZATION) by encapsulation within liposomes.
Certain drugs may be encapsulated within liposomes e.g. to protect them from metabolic degradation and/or to prevent them
from exerting general toxicity when delivered into the bloodstream; the liposomes fuse with or are endocytosed by cells of
the reticuloendothelial system, where they release their contents.
[Potential of liposome-mediated antiviral therapy: Antiviral Res.
(1985) 5 179190.] Drug-loaded liposomes can be targeted to
specific cells by the incorporation of antibodies to antigens in the
target cell surface; thus, e.g., immunoliposomes incorporating
a monoclonal antibody to herpes simplex virus glycoprotein D
were found to bind specifically to HSV-infected rabbit corneal
cells in vitro [J. Imm. (1986) 136 681685].
liposome swelling assay A method for determining the rate of
diffusion of ions or molecules through PORIN channels; purified
porins are incorporated into LIPOSOMES, and the rate of influx of
specified ions or molecules is estimated from the effects of the
(osmotically-induced) influx of water. [Method: JB (1983) 153
241252.]
lipoteichoic acid See TEICHOIC ACIDS.
Lipschutz
body An intranuclear inclusion body formed (late in
infection) in cells infected with e.g. herpes simplex virus type 1
or 2.
lirella (lirelliform apothecium) (lichenol.) A slit-like (long, narrow) apothecium; lirellae may appear as black branched or
unbranched lines with (in Graphis spp) or without (in Opegrapha spp) raised margins.
lirelliform apothecium Syn. LIRELLA.
lissamine rhodamine (acid rhodamine B; also: sulphorhodamine B) A red FLUOROCHROME (fluorescence: orange-red) used
for labelling proteins; it is initially treated with phosphorus
pentachloride and acetone to form the highly reactive sulphonyl
chloride derivative, and proteindye conjugation is then effected
by a sulphamido condensation.
Listeria
A genus of Gram-positive, asporogenous, aerobic/
facultatively anaerobic bacteria. Cells: rods or coccobacilli
(ca. 0.5 0.52 m), occurring singly or in small groups
(Chinese letter arrangements), palisades or filaments. Optimum
temperature range: 2537 C; growth occurs slowly at 4 C. Most
strains catalase +ve. Oxidase ve. Indole ve. Aesculin is
hydrolysed. Sugars are fermented to acid (no gas). Generally
motile. Colonies of L. monocytogenes: grey, translucent, about
1 mm in diameter after 2448 hours; a characteristic bluish
colour in obliquely transmitted light. L. monocytogenes may
give clear haemolysis on e.g. horse- and/or sheep-blood agar.
Listeria spp occur (apparently as saprotrophs) e.g. in soil,
decaying plant matter, silage, etc., and have been isolated from
e.g. faeces of healthy humans and animals; some haemolytic
strains of Listeria can be pathogenic in man and also in
animals (see LISTERIOSIS and MENINGITIS). [Wild birds and silage
as reservoirs of Listeria in the agricultural environment: JAB
(1985) 59 537543.] [The pathogenicity of L. monocytogenes
(a public health perspective): RMM (1997) 8 114.]
Some (human) infections with L. monocytogenes have been
linked to the ingestion of certain types of cheese. One approach
to the control of L. monocytogenes in cheese (during manufacture) involves the use of specific types of starter culture [see e.g.
AEM (1998) 64 48424845; JAM (1999) 86 251256].
Listonella
littoral A term used with different meanings by different authors;
thus, the littoral region of the marine benthic zone is variously
regarded as e.g. (a) the intertidal region, i.e., the zone which
is uncovered at low tide and under water at high tide; (b) a
zone below the average low-tide mark which is uncovered only
occasionally; (c) that region between the high-tide mark and
a depth of 200 metres. In freshwater environments the littoral
region may refer to those parts of the benthic zone which occur
in shallower waters of unspecified depth.
LIV-I binding protein See BINDING PROTEIN-DEPENDENT TRANSPORT SYSTEM.
live vaccine Any VACCINE containing viable, usually attenuated,
microorganisms (see e.g. BCG and STERNE STRAIN).
liver of sulphur See SULPHUR.
liver-stage-antigen 1 See MALARIA.
liverwort symbioses See e.g. NOSTOC and MYCORRHIZA.
lividomycin Either of two AMINOGLYCOSIDE ANTIBIOTICS (lividomycins A, B), both of which may be regarded as derivatives of
NEOMYCIN B.
Lk Linking number: see DNA.
LktA (of Pasteurella haemolytica) See RTX TOXINS.
LMD Culture Collection, Laboratory of Microbiology, Julianalaan 67A, 2628 BC Delft, The Netherlands.
lmp genes (EBV) See EPSTEINBARR VIRUS.
LmrA (Lactococcus lactis) See ABC TRANSPORTER.
lobar pneumonia See PNEUMONIA.
Lobaria
A genus of foliose LICHENS (order PELTIGERALES).
Photobiont: Myrmecia (in e.g. L. pulmonaria) or Nostoc (in
e.g. L. scrobiculata); Myrmecia-containing species may have
Nostoc-containing cephalodia cephalodia being fruticose in
L. amplissima (see CEPHALODIUM). Thallus: large (e.g. up to ca.
20 cm across), lobed, both surfaces corticate; the underside is
usually more or less tomentose, often with glabrous patches,
and in L. linita and L. pulmonaria the upper surface is coarsely
reticulate. Soredia may be present in e.g. L. pulmonaria and
L. scrobiculata. Apothecia: lecanorine, usually with reddish or
brown discs, abundant (in e.g. L. laetevirens) or scarce. Found
on rocks, bark etc, and generally very sensitive to air pollution.
Loboa A genus of fungi (? ENTOMOPHTHORALES). L. loboi causes
LOBOMYCOSIS and has not been cultured in vitro. In tissues,
it occurs as spherical, thick-walled, hyaline, yeast-like cells
(ca. 512 m diam.) which reproduce by budding; sequential
budding may lead to the formation of chains of cells.
lobomycosis (keloidal blastomycosis) A MYCOSIS, which apparently affects only man and dolphins, caused by Loboa loboi ; it
occurs in Central and South America. Infection is presumed to
occur via wounds; chronic, nodular, keloidal (elevated and scarlike) skin lesions develop chiefly (in man) on exposed areas of
the body.
lobopodium See PSEUDOPODIUM.
lobose pseudopodium See PSEUDOPODIUM.
Lobosea A class of naked and testate amoebae (superclass
RHIZOPODA) which form either lobopodia or filiform subpseudopodia from a broader hyaline lobe. The cells are typically
uninucleate; the few multinucleate members do not form plasmodia. Fruiting structures do not occur, but many members can
form resistant cysts. Orders: AMOEBIDA, ARCELLINIDA, PELOBIONTIDA, SCHIZOPYRENIDA, TRICHOSIDA.
lobster diseases See e.g. BURNED SPOT DISEASE and GAFFKAEMIA.
local lesion (plant virol.) A discrete lesion (e.g. a patch of
chlorosis or necrosis, or a RINGSPOT) which develops as a result
of localized viral infection in a leaf, stem etc. A plant which
readily develops local lesions when infected with a given virus
may be used for assaying that virus, and is termed a local lesion
host (= assay host ); the number of infective virus particles
present in a preparation can be assessed from the number of
lesions produced when the leaves of a suitable local lesion host
are inoculated with a known volume of the preparation. (See
also PLANT VIRUSES.)
Lockes solution A solution of inorganic salts used e.g. as a
liquid overlay for certain solid media. [Recipe: Book ref. 53, p.
2175.]
lockjaw Syn. TETANUS.
locomotor fringe Syn. TROCHAL BAND.
locule (loculus) A small chamber or cavity: see e.g. ASCOSTROMA
and FORAMINIFERIDA.
Loculoascomycetes A class of ascomycetes characterized by the
formation of bitunicate asci in ascostromata; the genera include
e.g. Elsinoe, Mycosphaerella, Myriangium and Venturia. The
class is not recognized in most modern taxonomic schemes.
locus (genetics) The position of a given gene, operon, mutation
etc on a chromosome, plasmid, or other genetic molecule.
locus of enterocyte effacement See PATHOGENICITY ISLAND.
Lodderomyces
A genus of yeasts (family SACCHAROMYCETACEAE). Cells are spheroidal, ellipsoidal, or cylindrical, and
reproduce by multilateral budding; pseudomycelium may be
formed. Asci are persistent. Ascospores: smooth, oblong to
fusiform, 1 or 2 per ascus. One species, L. elongisporus, isolated
e.g. from fruit juice and soil. [Book ref. 100, pp. 263265.]
lodging (plant pathol.) The collapse of cereal plants due to
bending or breaking of the stems; lodging may occur in certain
diseases.
Loefflers methylene blue See METHYLENE BLUE.
Loefflers serum A solid medium, usually prepared as a slope,
used e.g. for the culture of Corynebacterium diphtheriae. The
medium contains sterile serum and nutrient broth (3:1 by
volume) and glucose (ca. 0.250.5% w/v); this mixture may
be coagulated by TYNDALLIZATION or, if precautions are taken to
prevent foaming, by autoclaving.
log dilutions See SERIAL DILUTIONS.
log phase (of growth) See BATCH CULTURE.
logarithmic phase (of growth) See BATCH CULTURE.
Lolium enation virus See FIJIVIRUS.
lomasomes Membranous tubular, vesicular or sac-like structures
which occur, generally between the cell wall and cytoplasmic
membrane, in many fungi; they may be formed by invagination
of the cytoplasmic membrane, and often contain particulate
matter. The function of lomasomes is unknown; they have been
implicated e.g. in cell wall synthesis.
lon gene In Escherichia coli, a gene which encodes an ATPdependent protease that e.g. inactivates the SulA (= SfiA)
protein (see SOS SYTEM); the Lon protein is a HEAT-SHOCK PROTEIN.
long-incubation hepatitis Syn. HEPATITIS B.
longitudinal binary fission See BINARY FISSION.
longus A large plasmid-encoded fimbria (up to 20 m in length)
formed by strains of ETEC. The appendage consists of a repeated
22 kDa subunit, the N-terminal sequence of which shows some
homology with that of the subunits of various type IV FIMBRIAE
(including the TCP of Vibrio cholerae and bundle-forming pili
of EPEC). [Mol. Microbiol. (1994) 12 7182. In this paper the
appendage is referred to as a pilus.]
lonomycin See MACROTETRALIDES.
loop An instrument widely used in bacteriology and mycology
for the manipulation of small quantities of solid or liquid
material e.g. during INOCULATION; the rod-shaped metal handle
holds a piece of platinum or nickelsteel wire (310 cm long)
445
Lyme disease
LV agar See EGG-YOLK AGAR.
lyases ENZYMES (EC class 4) which catalyse either the nonhydrolytic removal of a group from a substrate with the
resulting (sometimes transient) formation of a double bond,
or the reverse reaction; when the reverse reaction is the
more significant (physiologically) the enzyme is often called
a SYNTHASE. Subclasses are recognized on the basis of the
nature of the bond split: e.g., CC, CO or CN. Lyases
include e.g. decarboxylases, aldolases and dehydratases. (See
e.g. HYALURONATE LYASE and PECTIC ENZYMES.)
Lyb antigens In mice: antigens which occur on certain mature
B lymphocytes. Lyb 5+ cells can respond to polyclonal B
cell activators (e.g. LPS) and also to soluble polysaccharide
antigens (e.g. certain bacterial capsular antigens); Lyb 5 cells
can respond to polyclonal B cell activators but not to soluble
polysaccharides.
Lycogala
A genus of slime moulds (class MYXOMYCETES) in
which the fruiting bodies are aethalia. L. epidendrum a common species on rotting logs forms clusters of hemispherical, puff-ball-like, pink to yellowish-brown aethalia, each ca.
0.31.5 cm diam.
lycomarasmin A TOXIN produced by certain strains of Fusarium
oxysporum (e.g. some strains of F. oxysporum f. sp. lycopersici,
the causal agent of FUSARIUM WILT in tomatoes). It chelates metal
ions, and at high concentrations can cause wilting in plants;
however, its role in pathogenesis if any is unknown.
lycopene See CAROTENOIDS.
Lycoperdales An order of fungi (class GASTEROMYCETES) in
which the basidiocarp consists of highly convoluted, hymeniumbearing fertile tissue enclosed by a peridium composed of two
or more layers; the organisms are characteristically humicolous
or lignicolous saprotrophs.
The so-called earth stars (e.g. Geastrum) form globose or
onion-shaped basidiocarps ca. 210 cm in diameter. When the
basidiocarp is mature, the exoperidium (the outer layer(s) of
the peridium) ruptures and peels back to form a stellate fringe;
in Geastrum, an apical pore develops in the remaining peridium (endoperidium) to permit spore release. (In Myriostoma
coliformis many pores develop in the endoperidium.)
The (non-stipitate) puffballs include species of Bovista,
Calvatia and Lycoperdon. In Calvatia spore release depends
on peridial rupture and disintegration; C. gigantea (the giant
puffball) may reach ca. 1 metre across. In Lycoperdon the spores
are released via a pore which develops in the peridium.
Lycoperdon See LYCOPERDALES.
lycoperdon nut A hypogean fruiting body of a member of the
Elaphomycetales.
Lyells syndrome Syn. SCALDED SKIN SYNDROME.
Lyme disease (Lyme borreliosis) A disease of humans (and e.g.
canines [VR (1995) 136 244247]) caused by Borrelia burgdorferi (see BORRELIA) and transmitted by the bite of (mainly ixodid)
ticks.
Symptoms (in humans): typically, an initial rash (erythema
migrans, EM) spreading from the tick bite, followed (after
days/weeks) by neurological/musculoskeletal/cardiac signs and,
later, joint/neurological/skin symptoms; symptoms vary in both
nature and timing.
Diagnosis: mainly serological (ELISA) (seroconversion after
4 weeks); detection of spirochaetes e.g. by culture or PCR
examination of blood.
Chemotherapy: e.g. ampicillin (during EM), ceftriaxone (for
arthritis, cardiac infection). Failure of chemotherapy may be due
to inaccessibility to antibiotics of intracellular spirochaetes [see
e.g. AAC (1996) 40 15521554].
lymphadenitis
basis of the predominant cell type involved and on the degree
of differentiation of the neoplastic tissue. (See also BURKITTS
LYMPHOMA, BOVINE VIRAL LEUKOSIS, MAREKS DISEASE.)
lymphomatosis A condition in which multiple lymphomas are
formed.
lymphon An individuals entire immune system, including e.g.
lymphoid tissues, LYMPHOCYTES, MACROPHAGES, and the COMPLEMENT system.
lymphopoiesis The development of LYMPHOCYTES.
lymphoproliferative virus group See GAMMAHERPESVIRINAE.
lymphosarcoma See SARCOMA.
lymphotactin (chemokine) See CHEMOKINES.
lymphotoxin a Syn. Tumour necrosis factor-b (TNF-b).
lymphotoxin b A membrane-anchored glycoprotein related to,
but distinct from, TNF-a and TNF-b.
lymphotropic virus group See GAMMAHERPESVIRINAE.
lymphotropism See TROPISM (sense 2).
Lyngbya A genus of freshwater and marine cyanobacteria of
the LPP GROUP. L. majuscula is responsible for causing dermatitis in swimmers (swimmers itch) e.g. in waters off the coasts
of Hawaii and Japan; this species can produce several toxins,
including the brominated phenolic aplysiatoxin, various derivatives of aplysiatoxin (e.g. debromo-, bromo and dibromoaplysiatoxin [structures: PAC (1986) 58 339350 (345)]), the indole
alkaloid lyngbyatoxin A, etc. (See also GEOSMIN and PHORMIDIUM.)
lyngbyatoxin See LYNGBYA.
lyophilization Syn. FREEZE-DRYING.
lysate The product of cell lysis.
lysergic acid diethylamide See ERGOT ALKALOIDS.
lysigenous (lysigenic) Syn. LYSOGENOUS.
lysin An antibody or other entity which, under appropriate conditions, can cause the lysis (rupture) of cells. See e.g. HAEMOLYSIN.
lysine biosynthesis See AMINOADIPIC ACID PATHWAY and DIAMINOPIMELIC ACID PATHWAY.
lysine decarboxylase test See DECARBOXYLASE TESTS.
lysis from without Lysis of a host cell when large numbers of
virions adsorb to the host cell surface. (See e.g. T-EVEN PHAGES.)
lysis inhibition In certain bacteriophages (e.g. T-even phages,
RNA phages): a delay in the lysis of an infected host cell on
superinfection of the cell with another phage of the same strain.
Mechanism: unknown. Lysis inhibition results in the formation
of plaques which each have a turbid halo. (cf. RAPID LYSIS
MUTANT.)
lysis protein (1) (syn. holin) A bacteriophage-encoded protein
that forms a pore in the cytoplasmic membrane of an infected
bacterium, thus enabling an ENDOLYSIN to gain access to the
peptidoglycan. In bacteriophage l, for example, a holin is
encoded by gene S ; this protein oligomerizes in the cytoplasmic
membrane, forming lesions which apparently allow the R gene
product to reach peptidoglycan [JB (1990) 172 912921]. The
requirement for the S gene product in bacteriophage l apparently
reflects the absence of a signal sequence (see SIGNAL HYPOTHESIS)
on the peptidoglycan-degrading R gene product, i.e. the latter, by
itself, could not cross the cytoplasmic membrane and therefore
could not effect lysis. In phage T4 the product of the t gene
appears to have the same role. In BACTERIOPHAGE f29 (which
infects Gram-positive bacteria), an analogous product is encoded
by gene 14 [JB (1993) 175 10381042].
In a phage-infected cell, a holin must be active only after
normal phage assembly has been completed; if lysis occurred
too early then fewer (or no) mature phages would be released
Lyssavirus
optimum of ca. 5.0. (The acidity within a lysosome is maintained
by a PROTON ATPASE in the lysosome membrane.) [The lysosome
membrane: TIBS (1986) 11 365368.] Lysosomes develop from
the distal end of the GOLGI APPARATUS; they are involved primarily in intracellular digestion: see AUTOLYSIN, FOOD VACUOLE,
PHAGOCYTOSIS. A primary lysosome is one which has not yet
coalesced with an autophagic or food vacuole or a phagosome;
following such coalescence the whole is termed a secondary
lysosome. When digestion is complete the entity remaining is
termed a residual body.
Certain viruses (e.g. Reovirus) depend on lysosomal enzymes
for uncoating.
Lysosomes may be damaged or disrupted e.g. by streptolysin
O or phalloidin.
lysostaphin A 22-kDa BACTERIOCIN produced by Staphylococcus
simulans (bv staphylolyticus) which is active against strains of
Staphylococcus aureus. Lysostaphin is an endopeptidase which
cleaves the glycylglycyl peptide bridges in staphylococcal
PEPTIDOGLYCAN, causing lysis. Immunity to lysostaphin in the
secreting organism is apparently due to modification of its
own peptidoglycan by an enzyme encoded by the lif gene.
Lysostaphin has been investigated for use in reducing numbers
of staphylococci in the nose and throat of carriers and for
the treatment of staphylococcal infections resistant to b-lactam
antibiotics.
lysozyme (N-acetylmuramidase; endolysin; endo-b-N-acetylmuramide glycanhydrolase; EC 3.2.1.17) An enzyme which hydrolyses the N-acetylmuramyl-(1 4)-b-linkages in PEPTIDOGLYCAN; it can thus cause BACTERIOLYSIS in species whose
peptidoglycan is accessible to enzyme action. (Micrococcus
luteus formerly M. lysodeikticus is particularly susceptible
and is used in lysozyme assays.) Lysozyme is widely distributed
in nature. Animal lysozyme (MWt ca. 14500; IEP ca. 11)
occurs e.g. in egg-white, milk, saliva, tears, mucosal secretions,
macrophages etc (cf. NON-SPECIFIC IMMUNITY). Structurally
distinct enzymes are produced by some bacteria and are coded
for by certain bacteriophages (e.g. T2, T4, l). An extracellular
lysozyme-like enzyme (endo-b-N-acetylglucosaminidase, EC
3.4.99.17, which cleaves the glucosaminidyl-(1 4)-b-linkages
in peptidoglycan) is produced by most coagulase-positive
and some coagulase-negative staphylococci [Book ref. 44,
pp. 746748].
lyssa Syn. RABIES.
Lyssavirus (rabies virus group) A genus of viruses within the
RHABDOVIRIDAE; type species: RABIES virus. The rabies virus is
neurotropic; the amino acid sequence of the virion glycoprotein
has been shown to resemble that of certain snake venom
curaremimetic neurotoxins which bind to acetylcholine receptors
on nerve cells [Science (1984) 226 847848]. The rabies
virus can multiply in nearly all types of mammalian and
avian cells in culture; it apparently replicates in the host
cell cytoplasm, budding predominantly from intracytoplasmic
membranes. Unlike VSV (see VESICULOVIRUS), it does not inhibit
cellular macromolecule synthesis. (See also FIXED VIRUS; FLURY
VIRUS; STREET VIRUS.)
The genus currently contains seven genotypes all of which,
except Lagos bat virus, are able to cause death in humans and/or
animals in nature; the genotypes are:
when the cell burst (i.e. the BURST SIZE would be affected). Such
early lysis was reported with a strain of phage l containing a
mutant S gene [Mol. Microbiol. (1994) 13 495504].
In some holin-encoding genes there are two start codons
(separated by one or two codons), i.e. the gene encodes two
polypeptides of slightly different length. The shorter product is
the holin, while the longer polypeptide seems to be an inhibitor
of holin activity; this arrangement may be a mechanism for
controlling the timing of cell lysis [Mol. Microbiol. (1996) 21
675682].
(2) The product of the lysis gene in a colicin plasmid (see
COLICINS).
(3) (syn. holin) A protein, product of the tcdE gene in
Clostridium difficile, which appears to promote the release
(across the cytoplasmic membrane) of toxin molecules (encoded
by genes tcdA and tcdB ) that lack a signal sequence [JMM
(2001) 50 613619].
Lysobacter
A genus of unicellular GLIDING BACTERIA; GC%:
6568. [IJSB (1978) 28 367393.]
lysochrome Any non-ionic coloured substance which dissolves
in and thus imparts colour to the lipids of cells or tissues. (See
e.g. SUDAN BLACK B and NILE BLUE A; cf. DYE.)
lysogen A lysogenic cell, or a population of lysogenic cells: see
LYSOGENY.
lysogenic (1) See LYSOGENY. (2) Syn. LYSOGENOUS.
lysogenic conversion See BACTERIOPHAGE CONVERSION.
lysogenic immunity See SUPERINFECTION IMMUNITY.
lysogenous (lysogenic; lysigenous; lysigenic) Refers to a structure, cavity or aperture (e.g. in a fungal fruiting body) which is
formed as a result of the breakdown of cells.
lysogeny The phenomenon in which the genome of a (temperate)
BACTERIOPHAGE establishes a stable, non-lytic presence in its
living host without producing progeny virions; the host cell
(which is said to be lysogenic) can continue to grow and
divide, and replication of the phage genome (the prophage) is
coordinated with that of the host chromosome such that, at each
cell division, the prophage is inherited by both daughter cells.
The prophage is maintained either by integration into the host
chromosome (as in the majority of temperate phages: see e.g.
BACTERIOPHAGE l, BACTERIOPHAGE MU and BACTERIOPHAGE f105)
or as an extrachromosomal plasmid (see e.g. BACTERIOPHAGE
P1 and BACTERIOPHAGE F116). (cf. PROVIRUS.) The host cell may
or may not exhibit an altered phenotype (see BACTERIOPHAGE
CONVERSION).
A prophage normally retains the potential to initiate a lytic
cycle in which progeny virions are produced and released by
cell lysis; maintenance of the lysogenic state necessitates the
repression of lytic functions in the prophage by means of phagedirected synthesis of a repressor protein (see e.g. BACTERIOPHAGE
l). (See also SUPERINFECTION IMMUNITY.) Derepression e.g. by
inactivation of the repressor protein results in induction of
the lytic cycle; induction may occur spontaneously in a small
proportion of cells in a lysogenic population. (See also ZYGOTIC
INDUCTION.)
(See also PSEUDOLYSOGENY and TRANSDUCTION.)
Lysol See PHENOLS.
lysopeptide Syn. signal peptide: see SIGNAL HYPOTHESIS.
lysophagosome See PHAGOCYTOSIS.
lysopine See CROWN GALL.
lysosome In eukaryotic cells (only): a closed, intracellular membranous sac (often ca. 0.5 m) containing a wide range of
enzymes which, collectively, can degrade various classes of
biological macromolecules; the enzymes typically have a pH
1.
2.
3.
4.
5.
449
Rabies virus
Lagos bat virus
Mokola virus
Duvenhage virus
European bat lyssavirus type 1
lysU gene
Lyt antigens Cell-surface antigens of murine T cells.
lytic bacteriophage Syn. VIRULENT BACTERIOPHAGE.
lytic cycle (virol.) The sequence of events which begins with
adsorption of a virus to a susceptible cell and terminates with
cell lysis and release of progeny virions.
lytic infection (virol.) The infection and subsequent lysis of
susceptible cells by a VIRUS. (cf. e.g. LYSOGENY.)
Lyticum
A genus of Gram-negative bacteria which occur as
endosymbionts in the cytoplasm of certain strains of Paramecium aurelia. Cells: peritrichously flagellated rods, ca. 0.60.9
2.010 m, which stain well with toluidine blue; in vitro cultivation has been reported. Lyticum spp do not contain R bodies
(cf. CAEDIBACTER) but they produce labile toxin(s) which lyse
sensitive paramecia. Type species: L. flagellatum.
L. flagellatum (earlier name: lambda particles) includes typically straight rods, while L. sinuosum (earlier name: sigma
particles) includes curved and spiral rods.
[Book ref. 22, pp. 808811.]
lyxose An aldopentose. (cf. STREPTOSE.)
450
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
M
m Maintenance coefficient: see YIELD COEFFICIENT.
M Methionine (see AMINO ACIDS).
M antigen (1) Streptococcal M PROTEIN. (2) A proteinLPS surface antigen in Brucella spp. (3) The COLANIC ACID capsular
antigen in certain enterobacteria.
M-associated protein See MAP.
M bands (of Stentor) See MYONEME.
M cells See DYSENTERY.
M fibres (of Stentor) See MYONEME.
M fimbriae FIMBRIAE which occur on some pyelonephritic strains
of Escherichia coli ; they bind to the amino-terminal part of
glycophorin AM .
M phase (of cell cycle) See CELL CYCLE.
M phenotype In strains of Streptococcus pyogenes and
S. pneumoniae: an efflux-based resistance to MACROLIDE
ANTIBIOTICS (q.v.).
M plasmid See MICROCINS.
M protein (1) (M antigen) (of streptococci) A heat-stable, trypsin-sensitive protein antigen associated with virulence in certain
(MC ) strains of group A streptococci. The M protein occurs
as a fibrillar fuzz covering the entire cell surface: the protein
molecules apparently occur in extended form as double-stranded,
a-helical coiled coils (ca. 50 nm long) anchored in the cell wall
by their C-terminal ends [PNAS (1981) 78 46894693]. The M
protein protects the cell from phagocytosis, and may play a role
in adhesion. MC strains often form matt or mucoid colonies on
solid media, and may under certain cultural conditions produce
an extracellular protease which degrades the M protein. M
protein occurs in different antigenic forms, providing a basis for
the serological typing of MC strains. (See also MAP; R PROTEIN;
T PROTEIN.)
(2) (in e.g. Escherichia coli ) The product of the lacY gene of
the LAC OPERON.
M ring See FLAGELLUM (a).
M1 RNA See RNASE P.
mAb Monoclonal antibody.
MAC (1) (immunol.) Membrane attack complex: see COMPLEMENT FIXATION.
(2) (bacteriol.) (syn. MAIS complex) Mycobacterium avium
complex: a category of slow-growing mycobacteria which
include M. avium, M. intracellulare and M. scrofulaceum. These
organisms are causal agents in three main types of infection:
(i) cervical adenitis in children, (ii) pulmonary disease in adults,
and (iii) disseminated disease in patients with advanced AIDS;
treatment for cervical adenitis involves resection of affected
node(s), while treatment for pulmonary and disseminated infections involves extended chemotherapy with a multiple drug
regimen that includes clarithromycin or azithromycin. [Infections due to MAC and their treatment: BCID (1997) 4 2561.
PCR-based detection of MAC bacteraemia in AIDS patients:
JCM (1999) 37 9094. Cross-reactivity between M. avium (and
M. kansasii ) and M. tuberculosis in AMTDT: JCM (1999) 37
175178.]
Mac-1 See INTEGRINS.
MacConkeys agar An agar-based medium used e.g. for the
primary isolation of Salmonella and Shigella from faeces, for
the differentiation of lactose-fermenting enterobacteria from
NLFs, etc. The medium contains (w/v): peptone (2%); lactose
(1%); sodium taurocholate or glycocholate (0.5%); NaCl (0.5%);
NEUTRAL RED (0.003%); agar (ca. 1.5%). Final pH: ca. 7.4.
Colonies of lactose fermenters (e.g. Escherichia coli ) are pink or
red, those of NLFs (e.g. most strains of Proteus, Salmonella and
Shigella) are colourless. Most non-enteric bacteria are inhibited
by the bile salts. Some commercial preparations also contain
crystal violet (1 mg/l) to inhibit Gram-positive bacteria.
MacConkeys broth A broth with the same formulation as
MACCONKEYS AGAR but without the agar. Bromcresol purple may
be used instead of neutral red as pH indicator.
Machupo virus See ARENAVIRIDAE and BOLIVIAN HAEMORRHAGIC
FEVER.
macrocapsule See CAPSULE.
macroconidium The larger of two types of CONIDIUM formed by
certain fungi (see e.g. FUSARIUM).
macroconjugant See CONJUGATION (1) (c).
macrocyclic rusts (eu-form rusts) (1) Those rust fungi (e.g.
Puccinia graminis) which form five clearly distinct types of
spore: pycniospores, aeciospores, uredospores, teliospores and
basidiospores (see UREDINIOMYCETES).
(2) Those rust fungi which form more than one type of binucleate spore i.e., aeciospores and/or uredospores in addition
to teliospores. (cf. DEMICYCLIC RUSTS.)
macrocyst A type of resting stage formed under certain conditions by (at least) some dictyostelid slime moulds (e.g. strains
of Dictyostelium discoideum, D. mucoroides, Polysphondylium
violaceum). It is formed when myxamoebae aggregate, and the
aggregate becomes enclosed in a fibrillar sheath; one of the cells
(the phagocytic or cytophagic cell) enlarges and begins to
engulf neighbouring amoebae. When all the peripheral amoebae
have been ingested, the remaining giant cell develops a cellulose
wall, its single large nucleus divides to form numerous smaller
nuclei, and the resulting multinucleate macrocyst enters a period
of dormancy. On germination, the macrocyst protoplast divides
into large, uninucleate proamoebae which in turn divide to
form normal-sized vegetative myxamoebae; these are released
when the macrocyst wall breaks down.
Macrocysts apparently represent a sexual stage in the dictyostelid life cycle. The large nucleus of the cytophagic cell is
believed to be that of a zygote; meiosis is presumed to occur
when this nucleus divides to form the multinucleate cyst.
[Review: Book ref. 144, pp. 178221.]
Macrocystis See PHAEOPHYTA.
macrodilution broth test See DILUTION TEST.
macrofibre In a culture of Bacillus subtilis grown under certain
conditions: a bundle of aligned chains of cells which can exhibit
a right-handed or left-handed helical conformation; the cell wall
in the cells of a helically twisted macrofibre is believed to
be under torsional stress. The helical conformation appears to
depend on the presence of intact glycan backbone chains (rather
than intact cross-links) in the cell wall PEPTIDOGLYCAN [JGM
(1986) 132 23772385].
macrogamete See ANISOGAMY.
macroglobulin (1) Syn. IgM (q.v.). (2) a2 -Macroglobulin is a
fibrinolysin inhibitor secreted by macrophages.
macrolide antibiotics A large group of MLS ANTIBIOTICS which
includes e.g. angolamycin, carbomycin, chalcomycin, cirramycin, erythromycin, lankamycin, leucomycin (D turimycin),
451
macronucleus
pathway from haemopoietic stem cells in the bone marrow, early
stages including the monoblast and MONOCYTE. [Macrophages:
JCS (1986) supplement 4, 267286.] Macrophages have important roles in host resistance to pathogenic microorganisms
(see PHAGOCYTOSIS, INFLAMMATION, ANTIBODY FORMATION and
DELAYED HYPERSENSITIVITY). (See also GIANT CELLS, HISTIOCYTE,
KUPFFER CELLS and PMN.)
Macrophages can express a wide range of cell-surface receptors, some of which are expressed constitutively while others can
be induced by appropriate stimuli. They include: (i) receptors
for the FC PORTION of IgG antibodies; (ii) receptors for various components of COMPLEMENT (e.g. CD46 and CD11c/CD18);
(iii) binding sites for lipopolysaccharides (see CD14); (iv) binding
sites for type I FIMBRIAE (see CD48); and (v) receptors for various
CYTOKINES.
Macrophages also display MHC class II molecules and
function as ANTIGEN-PRESENTING CELLS.
Under appropriate conditions (and with suitable stimulation), macrophages secrete a wide range of products, including:
(i) certain components of COMPLEMENT (e.g. FACTOR B, PROPERDIN, C1C5); (ii) FIBRONECTIN; (iii) certain PROSTAGLANDINS;
and (iv) various CYTOKINES (e.g. INTERLEUKIN-1, INTERLEUKIN-6,
INTERLEUKIN-8, INTERLEUKIN-12, INTERLEUKIN-18, TNF).
Activation of macrophages. On activation, a macrophage
e.g. (i) becomes more aggressive towards pathogens which
have been engulfed by phagocytosis, and (ii) secretes various
cytokines. Thus, an activated macrophage is associated with a
strong respiratory burst (see NEUTROPHIL) in which it produces
significant amounts of e.g. SUPEROXIDE, hydrogen peroxide and
NITRIC OXIDE; in the activated state a macrophage is able to kill
certain ingested pathogens which may not be killed in nonactivated macrophages.
Activation may occur e.g. when a macrophage presents antigen to an antigen-specific T LYMPHOCYTE of the Th1 subset
(this is an MHC class II-restricted interaction see HISTOCOMPATIBILITY RESTRICTION). Following such interaction with the
macrophage, the T cell secretes an important macrophageactivating factor: interferon-gamma (IFN-g) (see INTERFERONS).
IFN-g causes the macrophage to mount a respiratory burst (see
above) and to secrete cytokines such as IL-1, IL-6, IL-12, IL18 (see individual entries) and TNF-a (see TNF). Apparently,
IFN-g and lipopolysaccharides (LPS) can act synergistically to
enhance the respiratory burst [JBC (1990) 265 2024120246]
and to stimulate the synthesis of cytokines by macrophages. (The
ability of IFN-g and LPS to stimulate cytokine production in
macrophages may be inhibited by glucocorticoids.)
Cytokines secreted by a T cell may provide BYSTANDER HELP
(q.v.).
Following uptake, some pathogenic bacteria can kill macrophages [see e.g. EMBO (1996) 15 38533860; TIM (1998)
6 253255]; Yersinia down-regulates production of the proinflammatory cytokine TNF-a in macrophages [Mol. Microbiol.
(1998) 27 953965]. [Interactions between Mycobacterium
tuberculosis and phagocytes: TIM (1998) 6 328335.]
Macrophages may be maintained for some time in culture.
Viable macrophages adhere to glass and plastics and accumulate
dyes such as TRYPAN BLUE.
macrophage-activating factor See MAF.
macropinocytosis See DYSENTERY.
macroscopic Visible to the unaided eye.
macrostome See TETRAHYMENA.
macrotetralides A group of ANTIBIOTICS which function as
IONOPHORES; they inhibit Gram-positive bacteria. The cyclic
maize diseases
mal del pinto Syn. PINTA.
mal du coit Syn. DOURINE.
malachite green A green basic TRIPHENYLMETHANE DYE used e.g.
as an ENDOSPORE STAIN.
malaria An acute or chronic, sometimes recurrent, infectious
disease caused by species of PLASMODIUM and responsible, each
year, for some 12 million deaths (including many children);
the disease is prevalent in tropical and subtropical regions.
Malaria may be caused by Plasmodium falciparum, P. malariae,
P. ovale or P. vivax. (Mixed plasmodial infections can also
occur; moreover, P. knowlesi and P. simium, normally parasites
of non-human primates, can infect man under natural conditions,
causing simian malaria.)
Natural transmission of the malaria parasite from an infected
to an uninfected individual occurs via an insect vector: a
female mosquito of the genus Anopheles. [Systematics of malaria
vectors (in particular, the Anopheles punctulatus group): IJP
(2000) 30 117.] If, during a blood meal, the mosquito ingests
viable plasmodial gametocytes, male and female gametes can
develop and fertilization can take place in the insects gut; eventually, sporozoites forms of the parasite infective for a human
host appear in the salivary glands of the mosquito, and these
can be passed to an uninfected individual during the insects next
blood meal (see figure). [The malaria parasite in the mosquito:
PT (2000) 16 196201.]
Transmission may also occur e.g. by transfusion of infected
blood [NEJM (2001) 344 19731978].
Incubation period: ca. 728 days, or longer. The typical
illness is characterized by a series of paroxysms, each involving
an attack of rigors followed by high fever and then profuse
sweating. These paroxysms occur every 3648 hours in
falciparum malaria (malignant tertian malaria), 4248 hours
in vivax malaria (benign tertian malaria), 50 hours in ovale
malaria (tertian malaria), and 72 hours in malariae malaria
(quartan malaria). Other symptoms include e.g. headache,
malaise, nausea and vomiting, anaemia, and pains in the muscles,
joints and abdomen; enlargement of the liver and/or spleen may
occur.
Falciparum malaria exhibits the most severe symptoms, and
causes the majority of deaths from malaria. In certain blood vessels (the post-capillary venules), parasitized erythrocytes adhere
to endothelial cells although the significance of this in pathogenesis is not fully understood. Such adherence may lead to
mechanical obstruction of the vessels; it may, perhaps additionally, activate or damage endothelial cells and/or e.g. stimulate
the release of cytokines. Some authors indicate that disease manifestations result almost entirely from cytoadherence (adherence
of red blood cells to the endothelium) together with the induction of certain cytokines (TNF-a, IL-1 and IL-6) [BCID (1995)
2 227247]. In some cases, severe disease has been correlated
with a variant form of the TNF-a gene promoter [Nature (1994)
371 508510]. Another factor in falciparum malaria is rosetting: the phenomenon in which uninfected erythrocytes bind to
infected red cells; again, the significance of this in pathogenesis is not clear, although some studies suggest an association
between rosetting and cerebral malaria. Cytoadherence, rosetting
and impaired erythrocyte deformability have been discussed in
the context of abnormal microcirculatory blood flow [PT (2000)
16 228232]. Complications that may be associated with severe
malaria include anaemia, DISSEMINATED INTRAVASCULAR COAGULATION, hypoglycaemia and renal failure. (See also BLACKWATER FEVER.) [Pathogenesis of severe falciparum malaria: BCID
(1995) 2 249270.]
455
MALARIA. The life cycle of the malaria parasite (Plasmodium) (diagrammatic) showing the stages which are targets for antimalarial drugs (see table).
Sporozoites, injected into the bloodstream via mosquito bite, penetrate liver cells. A sporozoite grows and develops into a tissue schizont which undergoes asexual reproduction
(schizogony) to produce a number of cells called merozoites. On rupture of the liver cell, merozoites enter the bloodstream and infect erythrocytes (red blood cells). Within an
erythrocyte, a merozoite develops as a trophozoite (growing stage); the young trophozoite is known as the ring stage owing to its appearance in stained preparations under the
microscope.
The mature trophozoite (blood schizont) undergoes schizogony, and many merozoites are released [in a two-step process: PNAS (2001) 98 271276] when the erythrocyte
ruptures. These merozoites infect fresh erythrocytes. Some merozoites become gametocytes (i.e. cells with the potential to develop into male and female gametes). If ingested by a
mosquito, gametocytes give rise to gametes and the sexual phase of the life cycle follows.
In two species of Plasmodium the sporozoite can form a dormant stage (hypnozoite) in liver cells; hypnozoites may remain dormant for months/years. For this form of malaria a
radical cure involves treatment with an agent that kills hypnozoites (e.g. primaquine) as well as other drug(s) to deal with the intra-erythrocytic parasites.
Reproduced from Antimicrobial Drug Action, Figure 7.1, pages 120121, R. A. D. Williams, P. A. Lambert & P. Singleton (1996) copyright Bios Scientific Publishers Ltd, UK (ISBN
1-872748-81-3) with permission from the publisher.
malaria
Chemotherapy. Most antimalarials kill intraerythrocytic stages
of the parasite. The choice of drug(s) depends e.g. on the local
prevalence of parasites resistant to given antimalarials. (See
QUININE for the formulae of some antimalarials.)
Fansidar (D PYRIMETHAMINE C sulphadoxine) is an oral
treatment for uncomplicated falciparum malaria.
Quinoline-type antimalarials include QUININE, quinidine (used
e.g. in the USA), chloroquine and mefloquine (see AMINOQUINOLINES). Parenteral quinine is considered to be the drug of choice
for severe falciparum malaria because few strains of the parasite
are resistant to this form of treatment.
Chloroquine is used orally for uncomplicated falciparum
malaria and for most cases of vivax and ovale malaria.
Mefloquine is used orally for uncomplicated malaria and,
via nasogastric tube, for severe malaria; neuro-psychiatric sideeffects of this drug may be important [BMJ (1995) 310
709714].
Halofantrine is used orally for uncomplicated malaria. This
drug (9-phenanthrene methanol), unlike e.g. quinine, seems to
be active against the ring-stage trophozoite. The mechanism of
action is unknown. Halofantrine is not used for prophylaxis
owing e.g. to variable absorption. High levels of the drug have
been (rarely) linked with cardiac arrhythmias [Lancet (1993) 341
10541056].
Atovaquone (hydroxynaphthoquinone) is a candidate oral
antimalarial. It appears to inhibit electron transport in the
parasite.
Primaquine (an 8-aminoquinoline) is active against hypnozoites (but not against blood forms) and is used to prevent relapse
in vivax and ovale malaria; for a radical cure, primaquine is
used in conjunction with e.g. chloroquine.
WR238605 (a primaquine analogue) is being developed by
the US army (Walter Reed Army Institute of Research). It has
shown success in animal systems.
ANTIMALARIAL DRUGSa
Drug
Chemical description
Active againstb
Artemisinin
Sesquiterpene lactone
endoperoxide
Hydroxynaphthoquinone
4-Aminoquinoline
9-Phenanthrene methanol
4-Aminoquinoline
8-Aminoquinoline
Diguanide
Diaminopyrimidine
Quinoline-type (alkaloid)
Quinoline-type (alkaloid)
Sulphonamide
8-Aminoquinoline
BS
BS
BS
RS?
BS
TS, HYP
TS, BS
BS
BS
BS
BS
HYP, GAM
Atovaquonec
Chloroquine
Halofantrine
Mefloquine
Primaquine
Proguanil
Pyrimethamine
Quinidine
Quinine
Sulphadoxine
WR238605c
a
b
Mamiella
indicated, after 48 hours, by local oedema and a severe purulent
conjunctivitis.
Mallomonas
A genus of unicellular CHRYSOPHYTES which
resemble Chromulina spp but have a coating of silicified scales;
in some species the scales bear long siliceous spines.
malolactic fermentation A type of FERMENTATION (sense 2), carried out e.g. by species of Lactobacillus, Leuconostoc and Pediococcus, in which L-malic acid is converted to L-lactic acid and
CO2 . The reaction is apparently catalysed by a single enzyme
(the malolactic enzyme) which has no L-lactate dehydrogenase
activity; the malolactic enzyme from e.g. Lactobacillus plantarum has an absolute requirement for Mn(II) and NADC , but
the NADC is not reduced. There is no evidence that the reaction
yields ATP.
In certain fermented products (e.g. wines, pickled cucumbers,
soy sauce, silage) the malolactic fermentation has the effect
of reducing the acidity of the product (lactic acid being a
weaker acid than malic acid); this may or may not be desirable,
depending on the degree and nature of acidity required in
the product (see e.g. WINE-MAKING). Malolactic fermentation
in wine tends to be slow and may be unpredictable; where
required, it may be speeded up by the addition of a pure
culture of suitable bacteria (commonly Leuconostoc oenos).
The gene for malolactic fermentation has been transferred
from Lactobacillus delbrueckii to a wine yeast in an attempt
to produce a yeast capable of simultaneous malolactic and
alcoholic fermentations [AEM (1984) 47 288293]; however,
the resulting yeast exhibited only low levels of malolactic
fermentation.
Malpighamoeba A genus of amoebae (order AMOEBIDA). M. mellificae is parasitic in bees (see BEE DISEASES), M. locustae is
parasitic in locusts [Parasitol. (1976) 72 127135].
malt agar (malt extract agar) A medium made by diluting MALT
EXTRACT to a specific gravity of 10 Balling and solidifying it
with 2% agar.
malt extract An extract of malt, used e.g. as a medium for the
culture of a wide range of yeasts and moulds. Malt (1 kg) is
mixed with water (2.6 litres). The mixture is held at 45 C for
3 h (with stirring), and then at 63 C for 1 h; it is then filtered
and autoclaved. The specific gravity of the filtrate is adjusted
to 15 Balling using a Balling saccharometer. Malt extract is
available commercially in dehydrated form. (See also BREWING.)
Malta fever See BRUCELLOSIS.
Maltaner antigen A cardiolipinlecithin antigen used in certain
STANDARD TESTS FOR SYPHILIS.
maltase An a-glucosidase (EC 3.2.1.20) which hydrolysis (1 !
4)-a-D-glucosidic bonds; thus, e.g. maltose is converted to free
glucose.
maltobiose Syn. MALTOSE.
maltoporin See LAMB PROTEIN.
maltose (maltobiose) A reducing disaccharide: a-D-glucopyranosyl-(1 ! 4)-D-glucopyranose. Maltose is an intermediate in
the metabolic mobilization of STARCH in plants (e.g. during the
germination of cereal grains see e.g. BREWING); it also occurs
e.g. as a major product of photosynthesis in Chlorella symbionts
of Hydra viridis and of Paramecium bursaria (although it is not
produced by the non-symbiotic alga). Maltose can be metabolized
by a wide range of microorganisms. (For maltose transport in
e.g. Escherichia coli see BINDING PROTEIN-DEPENDENT TRANSPORT
SYSTEM.) (cf. ISOMALTOSE; see also AMYLASES and MALTASE.)
maltotriose A trisaccharide: a-D-glucopyranosyl-(1 ! 4)-a-Dglucopyranosyl-(1 ! 4)-D-glucopyranose. (See also AMYLASES.)
Mamiella See MICROMONADOPHYCEAE.
Proguanil (D Paludrine, CHLORGUANIDE) is a FOLIC ACID ANTAwith e.g. chloroquine it is used for prophylaxis. Of alternative prophylactic agents, mefloquine is absolutely contraindicated in early pregnancy.
See also QINGHAOSU.
In general, while antimalarials are used prophylactically by
travellers, such use is considered undesirable for residents in
endemic areas because it lowers the level of acquired resistance,
resulting in high mortality when the drug is withdrawn.
[Chemotherapy: Book ref. 213, pp 119128.]
[Malaria feature (vaccines, drugs, mosquito engineering etc.):
Science (2000) 290 428441.]
malarial pigment Syn. HAEMOZOIN.
Malassezia (syn. Pityrosporum)
A genus of non-fermentative
imperfect yeasts (class HYPHOMYCETES) which occur on the skin
in man and animals. The cells are spherical, oblong-ellipsoidal,
or cylindrical, and reproduce by monopolar bud-fission. True
hyphae are formed infrequently in culture, but are common
in skin scales. Growth is commonly stimulated by certain
oils (e.g. olive oil); optimum growth temperature: 3537 C.
The organisms can grow on glucose-peptone-yeast extract agar
(overlaid with olive oil for M. furfur ); they do not grow in the
liquid media used in standard physiological tests for yeasts. Two
species are recognized [Book ref. 100, pp. 882885]: M. furfur
(including Pityrosporum ovale and P. orbiculare, which are
currently considered to be variant cultural forms of M. furfur ),
and M. pachydermatis (D P. pachydermatis, P. canis). M. furfur
occurs e.g. on human skin (see also PITYRIASIS VERSICOLOR);
M. pachydermatis has been isolated from the ears of dogs
(in which it may be associated with otitis externa) and from
human skin.
malate synthase See TCA CYCLE.
male-specific phage Syn. ANDROPHAGE.
malic enzyme (1) See TCA CYCLE. (2) Syn. malolactic enzyme
(see MALOLACTIC FERMENTATION).
malignant (med.) (1) (of disease) Becoming progressively worse
(when untreated), usually resulting in death. (2) (of tumours)
Refers to a neoplasm which invades adjacent tissues and which
may metastasize (see METASTASIS). (cf. CANCER.)
malignant catarrhal fever (gangrenous coryza) An acute CATTLE DISEASE caused by a cytomegalovirus-like herpesvirus (see
BETAHERPESVIRINAE). The disease is characterized by high fever
with severe inflammatory and degenerative lesions in the mucous
membranes of the upper respiratory tract and intestinal tract; the
eyes may be affected, and blindness may result. Mortality rates
are generally high (usually >95%). The disease may also affect
certain other ungulates (e.g. sheep, wildebeest, deer). [Review
of the disease: VR (1984) 114 581583.]
malignant oedema (vet.) Tissue oedema and necrosis, often
involving frank GAS GANGRENE, due to wound infection by one
or more species of Clostridium e.g. C. chauvoei, C. novyi,
C. septicum, C. sordellii. Symptoms: fever, with a soft, red, local
swelling which becomes dark; in some cases gas production
gives rise to a frothy exudate from the wound. Death usually
occurs within 12 days. Treatment: parenteral administration of
antibiotics, antitoxin therapy (appropriate only in early stages of
the disease), irrigation of the wound with hydrogen peroxide.
(See also SWELLED HEAD.)
malignant pustule Cutaneous ANTHRAX.
malignant tertian malaria See MALARIA.
mallein test (vet.) A test for GLANDERS (sense 1) involving the
intradermal injection of mallein (containing antigens of the
pathogen) e.g. into the lower eyelid; a positive reaction is
GONIST;
457
Mancini test
maple bark strippers disease An EXTRINSIC ALLERGIC ALVEOLITIS associated with inhalation of the spores of Cryptostroma
corticale.
Maranil Dodecylbenzolsulphonate: an agent used e.g. in BTB
AGAR (0.005%) to inhibit swarming by Proteus spp.
Marasmius See AGARICALES (Tricholomataceae); see also MYCORRHIZA.
marble bone Syn. OSTEOPETROSIS.
marble spleen disease A disease of pheasants caused by an
adenovirus very similar to the causal agent of HAEMORRHAGIC
ENTERITIS OF TURKEYS. The disease is acute and rapidly fatal,
and involves severe pulmonary oedema with enlargement and
mottling of the spleen. [Book ref. 116, pp. 537539.]
Marburg fever (green monkey fever) A VIRAL HAEMORRHAGIC
FEVER, caused by the Marburg virus (see FILOVIRIDAE), first
reported in 1967 when an outbreak occurred in Marburg (W.
Germany) among laboratory personnel working with infected
tissues of the African green monkey (Cercopithecus aethiops).
Incubation period: ca. 610 days. Onset is sudden, with e.g.
fever, mental confusion, diarrhoea, haemorrhages from mucous
membranes, and often a maculopapular rash. The disease is often
fatal. (Ebola virus causes a similar disease.)
Marburg virus See FILOVIRIDAE.
Mareks disease (fowl paralysis) A POULTRY DISEASE caused
by gallid herpesvirus 1 (see GAMMAHERPESVIRINAE); chickens,
turkeys, pheasants, ducks, pigeons and other birds are susceptible, but the principal natural hosts appear to be domestic chickens and their close relatives (Gallus spp). Infection seems to
occur primarily by inhalation of feather dust released from the
feather follicles of infected birds. The classical (chronic) form
of the disease involves the development of T-cell lymphomas in
the peripheral nerves, causing progressive paralysis. A visceral
(acute) form also occurs in which lymphomas develop in internal
organs; mortality rates for the acute disease are commonly high.
Infected birds remain carriers probably for life. Live vaccines
are available: e.g., vaccination with gallid herpesvirus 2 (turkey
herpesvirus) protects chickens and turkeys against Mareks disease. [Review of Mareks disease and its virus: Book ref. 105,
pp. 155183.]
Mareks disease virus can also cause chronic atherosclerosis in
SPF chickens [AJP (1986) 122 6270]; MDV infection apparently prevents activation of cytoplasmic cholesteryl esterase in
arterial smooth muscle cells [JBC (1986) 261 76117614].
These observations lend support to the hypothesis that herpesvirus infection may play a role in the pathogenesis of
atherosclerosis (hardening of the arteries) in man [review: MS
(1986) 3 5052].
Marfanil (sulphamylon;
p-aminomethylbenzenesulphonamide:
NH2 CH2 .C6 H4 .SO2 .NH2 ) A drug which has been used e.g.
in the topical treatment of wounds, burns, etc. It differs from
other SULPHONAMIDES in that it is not a sulphanilamide derivative, the p-aminomethyl group replacing the p-amino group of
sulphanilamide.
marginal zone B cells (MZ B cells) A subset of B LYMPHOCYTES
found within the marginal zone of the spleen (i.e. the junction of red and white pulp) together with DENDRITIC CELLS and
macrophages; cells in the marginal zone are considered to represent an early form of defence against blood-borne pathogens.
MZ B cells are important in responses to T-independent antigens, and they are particularly sensitive to lipopolysaccharides.
[See e.g. Science (2000) 290 8992.]
Marinomonas See ALTEROMONAS.
Mastadenovirus
host sequences often undergoes amplification. Transformation
requires the integration of at least the E1a region, but the
mechanism of transformation is unknown. [Adenoviral genes
and transformation: Book ref. 110, pp. 125172.]
Human adenoviruses have been classified into subgenera (subgroups) on the basis of e.g. DNA characteristics, oncogenicity, subgenus-specific antigens, morphology, haemagglutinating
properties, etc:
Subgenus A (Ad12, 18 and 31): GC% of the DNA: 4749;
length of virion fibres: 2831 nm. Viruses in this subgenus
are highly oncogenic when injected into newborn hamsters or
rats, causing tumours after ca. 24 months; in man, they are
associated with upper respiratory tract infections and diarrhoea,
or infection may be subclinical.
Subgenus B (Ad3, 7, 11, 14, 16, 21, 34 and 35): GC%
of the DNA: 4952; length of the virion fibres: 911 nm.
Viruses in this subgenus are weakly oncogenic when injected
into newborn hamsters, causing tumours at low incidence after
ca. one year; in man, they cause e.g. ARD (Ad3, 7, 14, 21), acute
haemorrhagic CYSTITIS (Ad11), PHARYNGOCONJUNCTIVAL FEVER,
pneumonia, etc.
Subgenus C (Ad1, 2, 5 and 6): GC% of the DNA: 5759;
length of the virion fibres: 2331 nm. These viruses are nononcogenic in newborn rodents, but can cause transformation
of rodent cells in vitro; they can cause mild to severe upper
respiratory tract disease in young children.
Subgenus D (Ad810, 13, 15, 17, 19, 20, 2230, 32, 33, 36,
3739): GC% of the DNA: 5760; length of the virion fibres:
1213 nm. The viruses are non-oncogenic in newborn hamsters,
but may cause mammary adenomas in newborn female rats and
can transform rodent cells in vitro. Ad8 and Ad19 are causal
agents of EPIDEMIC KERATOCONJUNCTIVITIS.
Subgenus E (Ad4): GC% of the DNA: 57; length of virion
fibres: 17 nm. Non-oncogenic in newborn hamsters. Ad4 can
cause EPIDEMIC KERATOCONJUNCTIVITIS, acute respiratory disease
(see ARD), and PHARYNGOCONJUNCTIVAL FEVER.
Two further subgenera, F (Ad40) and G (Ad41), have been
recognized but are not yet well characterized; these include
the enteric or fastidious adenoviruses [review: Arch. Virol.
(1986) 88 117] which cause diarrhoea in infants and young
children, and which cannot be propagated in conventional cell
cultures. They can be grown in an Ad5-transformed human
embryonic kidney cell line.
Most human adenoviruses will not replicate readily in simian
cell lines, but may do so in the presence of simian virus 40
(SV40); SV40 can interact extensively with human adenoviruses,
e.g. forming SV40adenovirus hybrids [Book ref. 116, pp.
399449].
Animal adenovirus nomenclature follows at least two different
conventions; a species may be designated by a three-letter prefix
derived either from the name of the animal plus AV (e.g.
BAV for bovine adenovirus, SAV for simian adenovirus [Book
ref. 116, p. 500]) or from the genus name of the host animal
(e.g. bos for cattle, sus for pigs, equ for horses, mus for mice
[Book ref. 23, p. 60]), followed in either case by the serotype
(species) number e.g. BAV-3 or bos-3, MAV-1 or mus-1, etc.
Infection of animals by adenoviruses may result in (usually mild)
respiratory or diarrhoeal illnesses, conjunctivitis, etc. Canine
adenovirus type 1 (CAV-1, can-1) can cause encephalitis in foxes
and e.g. hepatitis in dogs; CAV-2 is thought to be a causal agent
of laryngotracheitis (kennel cough) in dogs. Several animal
adenoviruses (11 simian, 2 bovine and 2 canine species) can
induce tumours when injected into newborn hamsters. [Animal
adenoviruses: Book ref. 116, pp. 497562.]
Mastigocladus
maternal inheritance A form of CYTOPLASMIC INHERITANCE in
which certain characteristics are transmitted to sexually derived
progeny only from the female parent cell. Various hypotheses
have been proposed to account for maternal inheritance, and
different mechanisms may be applicable in different cases. Thus,
in certain cases where maternally inherited genes occur in
mitochondria, mitochondria from the male parent are presumed
to be excluded from the zygote (see e.g. POKY MUTANT). To
account for the maternal inheritance of genes in chloroplast DNA
(a phenomenon recorded in some isogamous green algae) it has
been proposed that chloroplast DNA from the male parent is
preferentially digested [MS (1985) 2 267270].
mating Syn. CONJUGATION (sense 1).
mating type A strain of an organism which can interact sexually
only with other, genetically distinct, strains of the same species.
(See also HETEROTHALLISM and SYNGEN.)
In Saccharomyces cerevisiae mating type is determined at a
single genetic locus, designated MAT, on chromosome III. In
haploid cells, MAT is occupied by either the MAT a allele or the
MAT a allele which occur in a and a mating types respectively.
According to the widely-accepted a1-a2 hypothesis, MAT a
and MAT a regulate the same groups of structural genes, but
their different modes of regulation result in the development
of phenotypically different mating types; thus, groups of genes
known as a-specific genes and a-specific genes (which
specify the a and a phenotypes, respectively) occur in the cells of
both a and a mating types, and the way in which these genes are
controlled by the MAT locus determines the cells mating type.
MAT a is transcribed in two parts from a central promoter
region, the two RNA transcripts being copied from different
DNA strands; the parts are called MAT a1 and MAT a2. MAT a1
expression is necessary for the transcription of the a-specific
genes whose products include the a-f actor (a PHEROMONE).
MAT a2 is a negative regulator of a-specific genes.
The (single) MATa product has no effect in the a-type haploid
vegetative cell; by default, a-type genes (including that encoding
the a-type pheromone a-factor) are expressed in cells of this
mating type.
In most natural isolates of S. cerevisiae, spontaneous conversion of the MAT a allele to the MAT a allele, and vice versa,
occurs quite frequently with concomitant switching of mating type; a given population will therefore consist of a mixture of compatible mating types (a and a) and will give the
appearance of being homothallic. (Stability at the MAT locus
involves another locus, designated HO for homothallism, located
on chromosome IV.) Switching involves a cassette mechanism,
unexpressed copies of MATa and MATa being stored on chromosome III at sites designated, respectively, HMR and HML;
these genes are silenced by the transcription-resistant form of
their chromatin. Switching requires a double-stranded cut at the
MAT locus, made by the HO (YZ) endonuclease, followed by
excision of the resident MAT allele and its replacement with a
copy of the allele of the other mating-type (gene conversion).
When a-type and a-type cells are mixed, the pheromone from
a given mating type causes cells of the other type to stop in
the G1 phase of the CELL CYCLE, and to exhibit a mating typespecific glycoprotein component of the cell wall which promotes
fusion between cells of opposite mating types. The zygote,
which lacks mating potential and mating type characteristics,
is designated a/a.
In the a/a zygote, the a2 and a1 proteins jointly switch off
various genes, including a-specific and a-specific genes and the
haploid-specific genes active in both mating types.
measles
between an ecotropic MuLV and an endogenous xenotropic
retrovirus. Since many MCF viruses have a leukaemogenic
potential greater than that of the parent MuLV, it has been
suggested that an MCF component may be responsible for
MuLV-induced leukaemogenesis. (See also AKV; cf. FRIEND
VIRUS.)
McFadyeans test A confirmatory test for ANTHRAX carried out,
post-mortem, on an infected guinea pig. Blood (from the heart),
or a spleen imprint, is stained with polychrome methylene blue;
in a positive test, the stained smear reveals large, blue, squareended bacilli surrounded by a reddish granular capsule.
McIntosh and Fildes anaerobic jar (modified) An ANAEROBIC
JAR which consists of a strong cylindrical metal chamber with
a flat, circular, gas-tight lid; such jars are referred to by various
trade names (e.g. Torbal jar). Media etc are placed in the jar, and
the lid is secured by means of a screw clamp. The jar is then
evacuated, by a suction pump, via one of two screw-controlled
needle valves in the lid; this valve is then closed. (To prevent the
vacuum sucking the agar from Petri dishes, plates are incubated
lid-side up cf. GASPAK.) The jar is filled, via the other valve,
with gas(es) e.g. H2 , or CO2 and H2 from a compressed-gas
cylinder or from a gas-filled rubber bladder; this valve is closed,
and the cycle of evacuation and re-filling is carried out several
times. Attached to the inside of the lid is a gauze envelope
containing a catalyst (e.g. palladium-coated pellets of alumina)
which promotes chemical combination between hydrogen and
the last traces of oxygen in the jar; such catalysts work at room
temperatures and are called cold catalysts. The jar also has
a side-arm to which is attached a small, thick-walled, closed
glass vessel which communicates with the interior of the jar
and which contains an indicator of anaerobiosis (e.g. METHYLENE
BLUE solution).
MCP (1) Methyl-accepting chemotaxis protein (see CHEMOTAXIS).
(2) Membrane co-factor protein (see COMPLEMENT FIXATION (b).)
MCS (multiple cloning site) See POLYLINKER.
M-CSF See COLONY-STIMULATING FACTORS.
MDa Megadalton: 106 DALTONS.
MDCK cells MadinDarby canine kidney cells: a heteroploid
cell line derived from the kidney of an apparently normal
dog. MDCK cell cultures have been used e.g. for the primary
isolation and passage of influenzavirus type A [PNAS (2000) 97
96549658].
MDP Muramyl dipeptide: N-acetylmuramyl-L-alanyl-D-isoglutamine; a water-soluble component of a modified form of
complete FREUNDS ADJUVANT.
mean doubling time See GROWTH (a).
mean generation time See GROWTH (a).
measles (morbilli; cf. RUBEOLA) An acute and highly infectious
human disease which affects mainly children. (Other primates
can be affected.) The causal agent is a MORBILLIVIRUS. Transmission occurs by droplet infection or via fomites; the conjunctivae
may be important sites of infection. Incubation period: 812
days. In the prodromal stage (24 days) there is coryza, cough,
fever, and the appearance of KOPLIKS SPOTS. Subsequently, a
maculopapular rash develops on the head, then on the limbs and
trunk. The spots are initially bright pink but become deeper red
and then brownish a phenomenon known as staining. Viruses
are present in the urine, nasopharyngeal secretions etc during the
prodromal period and for several days after the appearance of the
rash. Complications may include ENCEPHALITIS [NEJM (1984)
310 137141]; secondary bacterial infection may result in e.g.
meat spoilage
OTITIS MEDIA or PNEUMONIA. Measles is usually self-limiting,
but may be fatal in young infants or in malnourished children; death is usually due to respiratory complications. Life-long
immunity usually follows recovery (cf. SUBACUTE SCLEROSING
PANENCEPHALITIS). Lab. diagnosis: microscopic examination of
smears of the nasal mucosa for epithelial GIANT CELLS; detection of the measles virus in blood, urine or nasal secretions.
Chemotherapy: none. Measles immune globulin may be used
prophylactically in high-risk patients exposed to measles. Live
attenuated vaccines (cf. MR and MMR) may be given to infants
and young children.
meat spoilage The occurrence, nature and extent of meat
spoilage depends on e.g. the initial numbers and types of contaminating microorganisms, the conditions of storage (particularly
temperature and oxygen tension), the length of storage, and the
nature of the meat itself (e.g. its WATER ACTIVITY, glucose content
[see e.g. AEM (1982) 44 521524], pH). Spoilage may involve
slime formation, discoloration, souring, and off-odours (due e.g.
to the volatile products of microbial amino acid metabolism).
(a) Carcasses. Carcass meat is normally surface-contaminated
with bacteria and fungi derived from the animals skin, intestine,
faeces etc., from soil, and e.g. from the hands and tools of workers. Even under good hygienic conditions, carcasses are likely
to carry 102 105 bacteria/cm2 , but spoilage commonly becomes
apparent only after bacterial numbers reach ca. 107 109 per cm2 .
After slaughter, the pH of meat gradually falls as the muscle
glycogen is converted to lactic acid the final pH depending
on the amount of glycogen present at the time of death. The
final pH of red meats is commonly 5.45.8; chicken leg meat
normally has a pH of ca. 6.5, although the breast meat usually
has a pH of ca. 5.7. Meat from stressed animals has a higher pH
and is more susceptible to spoilage see DFD MEAT.
For short-term storage, carcasses may be chilled to e.g.
010 C. Below ca. 10 C psychrotrophic spoilage organisms
increase greatly in numbers; by contrast, pathogenic organisms
(cf. FOOD POISONING) grow very slowly, and their presence is
usually not obvious. In most meats, including uncured pig meat
and poultry, the commonest spoilage bacteria under aerobic conditions are strains of Pseudomonas [JAB (1982) 52 219228
(taxonomic study)], often occurring together with smaller numbers of bacteria such as Acinetobacter, Alteromonas, Brochothrix
and Lactobacillus spp. Of the spoilage organisms, Pseudomonas
spp have the highest growth rate at low temperatures, and this
advantage tends to become more marked with decreasing temperature. (In poultry, Acinetobacter replaces Pseudomonas as
the commonest spoilage organism at temperatures above ca.
10 C.) However, Brochothrix thermosphacta and Lactobacillus
spp, for example, are more tolerant than pseudomonads of low
aw , and these may become dominant on drying carcasses. On
cured meats (see CURING), e.g. bacon, the commonest spoilage
bacteria under aerobic conditions are halophilic, psychrophilic
vibrios (e.g. Vibrio costicola) and species of Acinetobacter and
Micrococcus; the micrococci are lipolytic and proteolytic, and
some strains can reduce nitrite. Fungi found on chilled carcasses
include Cladosporium, Penicillium, Mucor, Rhizopus and Thamnidium, and the yeasts Candida, Cryptococcus and Rhodotorula;
these may cause e.g. surface discolorations.
For long-term storage, temperatures of ca. 12 C to 18 C
are often used; the process of freezing kills or damages
a proportion of contaminants, although lower temperatures
(e.g. 30 C) are less lethal (see FREEZING). At temperatures
between ca. 5 C and 10 C fungal contaminants may become
important spoilage agents (see e.g. BLACK SPOT sense 1).
meiosis
medium In microbiology: any liquid or solid preparation made
specifically for the growth, storage or transport of microorganisms or other types of cell. Growth media for microorganisms may be used e.g. for the initiation of a CULTURE (or a
SUBCULTURE), for ENRICHMENT, or for diagnostic (identification)
tests i.e. tests in which the identity of a given organism may
be deduced from the characteristics of its growth in or on particular media. (See also TRANSPORT MEDIUM.) Specialized media
are used for the growth/maintenance of mammalian (and other)
cells in TISSUE CULTURE (q.v.). Before use, a medium is normally
STERILE (sense 1).
Many chemolithautotrophic bacteria can be cultured in simple
aqueous media containing mainly, or only, mixtures of inorganic
salts. Nutritionally undemanding heterotrophs can be grown
on/in a range of culture media (see e.g. NUTRIENT BROTH and
PETONE WATER). Nutritionally fastidious heterotrophs may be
grown on an ENRICHED MEDIUM. Strict anaerobes are often
cultured on prereduced media (see ANAEROBE).
Solid media usually consist of liquid media which have been
solidified (gelled) with an agent such as AGAR or GELATIN; other
gelling agents include e.g. ALGINATE, Gelrite (see GELLAN GUM),
and PLURONIC POLYOL F127. (See also SILICA GEL.) Solid media
(such as e.g. NUTRIENT AGAR) may be used in order to obtain
colonies (see COLONY) of a given organism; colonies may be
required for identification purposes or e.g. for the determination
of viable cell counts (see COUNTING METHODS). Media containing
an unusually high concentration of solidifying agent (e.g. stiff
AGAR) are used e.g. to inhibit SWARMING; those containing less
than normal concentrations of solidifying agent (e.g. semi-solid
or sloppy agar) may be used e.g. for CRAIGIES TUBE METHOD.
Basal medium. One which, without supplement, can support
the growth of various nutritionally undemanding species; see
e.g. NUTRIENT BROTH.
Defined medium. One in which all the constituents (including
trace substances) are quantitatively known.
Differential medium. A solid medium on/in which different
types of organism may be distinguished by their different forms
of growth; see e.g. MACCONKEYS AGAR; SS AGAR.
Diphasic medium. See DIPHASIC MEDIUM.
Enriched medium. See ENRICHED MEDIUM.
Enrichment medium. See ENRICHMENT MEDIUM.
Inhibitory medium. One containing certain constituent(s)
which suppress the growth of certain type(s) of microorganism.
Maintenance medium. One used for the initial growth and
subsequent storage (under conditions of minimal growth) of
microorganisms or other cells. For microorganisms, a maintenance medium is used to prepare a CULTURE of the given
organism which is then stored either at room temperature or
under refrigeration; subculture is required at intervals ranging
from 1 to 12 months. Ideally, the constituents of a maintenance
medium are the minimum consistent with the need to maintain
viability of the organisms. Examples: COOKED MEAT MEDIUM and
DORSETS EGG. (See also TISSUE CULTURE.)
Pre-reduced medium. See ANAEROBE.
Selective medium. One which allows or encourages the growth
of some type(s) of organism in preference to others. The
term usually refers to media such as DCA, MacConkeys agar
(which generally supports the growth of enteric but not nonenteric bacteria), and all the various types of enrichment
media; however, all media are selective to some extent.
Test medium. One used for diagnostic (identification) tests.
Test media are often made by incorporating additional substance(s) into standard or modified liquid or solid media; often a
463
meiosporangium
L-arabinose.
mercury
Unlike other lymphocytes in the circulation, memory cells persist for long periods of time; they are also distinguishable by
certain cell-surface antigens, e.g. CD44.
(See also ANTIBODY FORMATION.)
menadione See QUINONES.
menaquinones See QUINONES.
Mendosicutes A proposed division of the PROCARYOTAE comprising the single class ARCHAEOBACTERIA.
mengovirus See CARDIOVIRUS.
meningitis Inflammation of the meninges (membranes covering
the brain and spinal cord). Meningitis may be of non-microbial
causation, or it may result from primary or secondary infection
by any of a range of microorganisms which gain access to the
meninges via the blood or lymph systems, head wounds, or
paranasal sinuses.
(a) Bacterial meningitis. Symptoms typically include a severe,
throbbing headache, stiff neck, fever, delirium and coma;
bacterial meningitis may be rapidly fatal. Lab. diagnosis: the
pathogen can often be detected by microscopic examination of
a Gram-stained smear of CSF sediment.
Meningococcal meningitis (epidemic meningitis) caused
by Neisseria meningitidis (the meningococcus) occurs sporadically or in epidemics. Transmission occurs by direct contact or
by droplet infection; asymptomatic carriers harbour meningococci in the nasopharynx. Incubation period: ca. 210 days.
Onset is usually abrupt, with rapid progression to confusion
and coma; meningitic symptoms are often accompanied by
petechial or purpuric skin lesions which may become gangrenous. Mortality rates: ca. 2575% in untreated cases, ca.
710% in treated cases. A severe, fulminating form involving
cyanosis, coma, and skin and adrenal haemorrhages (WaterhouseFriderichsen syndrome) may be fatal within a few hours.
Chemotherapy: benzylpenicillin, chloramphenicol. Rifampicin
can eliminate meningococci from carriers. [A meningococcal C
vaccine in teenagers: Lancet (2003) 361 675676.]
Haemophilus influenzae type b is a common cause of bacterial meningitis in infants and young children, often secondary to
otitis media, pneumonia or viral respiratory disease. Mortality
rates (treated cases): ca. 310%. Chemotherapy: e.g. chloramphenicol.
Pneumococcal meningitis (caused by Streptococcus pneumoniae) occurs mostly in infants and the elderly or debilitated.
It is commonly associated with pneumococcal pneumonia, but
may follow otitis media, head wounds etc. Mortality rates: ca.
2070%. Chemotherapy: e.g. benzylpenicillin, chloramphenicol.
Various other bacteria can cause meningitis in adults e.g.
other streptococci, staphylococci, Acinetobacter calcoaceticus,
Listeria monocytogenes, enterobacteria. Neonates are particularly vulnerable to meningitis caused by Escherichia coli
and other enterobacteria, group B streptococci, Staphylococcus aureus, L. monocytogenes, Flavobacterium meningosepticum etc; mortality rates may be high, and motor or intellectual
impairment often persists in survivors.
(b) Aseptic meningitis is generally a benign, self-limiting
condition characterized by a lymphocytic infiltration of the
meninges and raised protein levels in the CSF. It is usually
caused by a virus commonly mumps virus or enteroviruses
(e.g. echoviruses or coxsackieviruses), also e.g. ENCEPHALITIS
viruses, herpes simplex virus and LCM VIRUS. A lymphocytic
meningitis may also occur in e.g. CRYPTOCOCCOSIS, LEPTOSPIROSIS, SYPHILIS and TUBERCULOSIS; following administration of
nerve-tissue rabies vaccines (e.g. Semple vaccine); and in certain non-microbial diseases (e.g. cerebral tumours). (See also
MENINGOENCEPHALITIS.)
meningococcus Neisseria meningitidis.
meningoencephalitis Inflammation of the brain and its meninges
(cf. ENCEPHALITIS and MENINGITIS). Primary amoebic meningoencephalitis is a human disease which affects mainly children and
young adults and is usually fatal. It is usually caused by Naegleria fowleri. Infection occurs via the nasal mucosa and is usually
associated with swimming in e.g. freshwater lakes rich in organic
matter. Symptoms may include headache, fever, vomiting, disturbances to taste, smell and vision, and coma; death may occur
within ca. 72 h. Amoebae of the Acanthamoeba-Hartmannella
group may cause a subacute or chronic granulomatous meningoencephalitis. Lab. diagnosis: identification of amoebae in the
CSF. Chemotherapy: e.g. amphotericin B (see also MICONAZOLE).
meningoencephalomyelitis See ENCEPHALITIS.
meningomyelitis Inflammation of the spinal cord and its meninges (cf. MENINGITIS).
Meniscus A genus of Gram-negative, anaerobic (but aerotolerant) bacteria which occur e.g. in anaerobic digester sludge.
The cells are capsulated, straight or curved, non-motile rods,
0.71.0 2.03.0 m, which contain gas vacuoles. The organisms are chemoorganotrophs with a strictly anaerogenic fermentative metabolism; growth requirements include vitamin
B12 , thiamine, and a raised partial pressure of CO2 . Optimum
growth temperature: ca. 30 C. GC%: ca. 45. Type species:
M. glaucopsis. [Book ref. 22, pp. 135137.]
Menoidium See EUGLENOID FLAGELLATES.
menthol See PHENOLS.
mepacrine Syn. QUINACRINE.
merbromin See MERCURY.
2-mercaptoethanesulphonic acid Coenzyme M: see METHANOGENESIS.
mercaptoethanol (HSCH2 CH2 OH) A reagent used e.g. to reduce
disulphide bonds in proteins (e.g. immunoglobulins see FAB
PORTION).
Mercurochrome See MERCURY.
mercury (as an antimicrobial agent) Mercury is a HEAVY METAL
whose compounds include many effective antimicrobial agents;
such agents are typically reversibly microbistatic, and they have
little or no effect on the viability of bacterial endospores though
they can delay germination. The functional part of an antimicrobial mercurial is the mercury cation or the mercury-containing
moiety; antimicrobial activity may involve the binding of these
entities to certain groups (particularly thiols but also e.g.
amides and amines, purines and pyrimidines) in e.g. enzymes,
cell walls, cytoplasmic membranes and nucleic acids. Microbistatic activity can be reversed with e.g. thiols which probably
compete with the mercury-binding sites of the organisms. In
bacteria, resistance to mercurials can be plasmid-mediated.
Inorganic mercurials are toxic and irritant to tissues; their
activity is readily inhibited or reversed by organic matter
(e.g. blood or serum). Mercuric chloride (corrosive sublimate)
has been used for the disinfection of inanimate objects when
other methods are unsuitable, and as a preservative for e.g.
paper and timber. Mercurous chloride (calomel) has restricted
use as a fungicide in horticulture e.g. as a control against
clubroot. Yellow mercuric oxide has been used in ointments
for the treatment of conjunctivitis and blepharitis. Ammoniated
mercury (aminomercuric chloride; white precipitate; HgNH2 Cl)
has been used in ophthalmic preparations and for the treatment
of superficial mycoses.
465
Methanobacteriaceae
produces depsipeptide entomotoxins (destruxins) which apparently play an important role in pathogenesis. M. anisopliae
has been used for the BIOLOGICAL CONTROL of e.g. froghoppers
(Mahanarva posticata) in Brazilian sugar-cane plantations.
metastasis (med.) The dissemination of disease from a localized
site in the body, with the formation of new foci at distant
sites. (Usually used in the context of CANCER, but also of
certain infectious diseases e.g. TUBERCULOSIS.) (Hence verb
metastasize, adj. metastatic.)
metatrypanosomes Syn. METACYCLIC FORMS.
Metchnikovella See RUDIMICROSPOREA.
methacycline See TETRACYCLINES.
metham sodium (vapam) Sodium N-methyl-DITHIOCARBAMATE
(CH3 .NH.CS.SNa), a soil fumigant which, in soil, breaks down
to form the volatile methyl-isothiocyanate. (cf. DAZOMET, QUINTOZENE.)
methanal Syn. FORMALDEHYDE.
methane monooxygenase (MMO) A MONOOXYGENASE which
occurs in methanotrophs (see METHYLOCOCCACEAE) and which
catalyses the oxidation of methane to methanol by molecular
oxygen; MMO can also catalyse the oxidation of substrates such
as n-alkanes and n-alkenes: e.g., propene (propylene) is oxidized
to 1,2-epoxypropane. (See also CO-METABOLISM.)
MMO may be particulate (i.e., membrane bound) or soluble,
depending on growth conditions. Thus, e.g., in cells of Methylococcus capsulatus and Methylosinus trichosporium grown on
methane, the MMO is soluble or particulate according to whether
the culture medium contains low (e.g. 1 M) or high (e.g.
5 M) levels of Cu2C respectively. However, in M. capsulatus
only particulate MMO is formed when growth occurs on
methanol in this case an increase in the level of Cu2C enhancing MMO activity [JGM (1985) 131 155163]. The soluble
MMO of M. capsulatus is a three-component enzyme comprising proteins A (believed to be the oxygenase [JBC (1984) 259
5359]), B and C, and that of Methylosinus trichosporium is
apparently similar.
The substrate specificities of particulate and soluble MMOs
may differ appreciably. Thus, e.g. the soluble MMO of
M. trichosporium can oxidize n-alkanes, n-alkenes, aromatic
and alicyclic compounds, while the particulate MMO of the
same organism cannot oxidize aromatic or alicyclic substrates
[JGM (1984) 130 33273333].
In various types of methanotroph the reducing power requirement for MMO activity in vitro (i.e. in cell extracts) appears
to be satisfied by NADH for both the soluble and particulate
forms of the enzyme. However, it has been proposed that the
reducing power needed for in vivo particulate MMO activity
in M. trichosporium may be derived from a reduced c-type
cytochrome. It has been suggested that reducing power for in
vivo particulate MMO activity in M. capsulatus may be supplied by an electron transfer protein (e.g. an FeS protein) the
reduction of which depends on reversed electron transport [JGM
(1983) 129 34873497].
methane production See METHANOGENESIS.
methane utilization See METHANOTROPHY.
Methanobacillus omelianskii A syntrophic association of two
species of prokaryote: Methanobacterium bryantii and an obligate proton reducer (the S organism) which oxidizes ethanol
to acetate and hydrogen gas.
Methanobacteriaceae A family of METHANOGENS (order
METHANOBACTERIALES); two genera: METHANOBACTERIUM and
METHANOBREVIBACTER. (This family formerly included all the
methane-producing species.)
Methanobacteriales
M. voltae. Cells ca. 0.53.0 m diam. Mesophilic. Growth is
optimal in 0.4 M NaCl. Methane is produced from carbon dioxide
and hydrogen and from formate.
methanofuran See METHANOGENESIS.
methanogen Any member of the domain ARCHAEA which can
carry out METHANOGENESIS; all known methanogens are obligate
anaerobes which occur e.g. in muds and in the RUMEN (some
forming close physical associations with protozoa [MS (1986) 3
100105]). (See also ANAEROBIC DIGESTION and WETWOOD.)
Methanogens have been classified in three orders (METHANOBACTERIALES, METHANOCOCCALES, METHANOMICROBIALES) on the
basis of 16S rRNA sequence analysis.
Many methanogens can grow chemolithoautotrophically in
mineral salts solution with carbon dioxide and hydrogen
(although some need e.g. acetate and amino acids). Methanogens
are not necessarily confined to simple substrates such as
acetate, methanol and methylamines; thus, pure cultures of e.g.
Methanospirillum can be grown on 2-propanol and certain other
alcohols [AEM (1986) 51 10561062].
The methanogens have been divided into two groups: group I
(carbon dioxide and hydrogen, or formate, typically used), and
group II (carbon dioxide and hydrogen, or formate, typically not
used); group II includes the family METHANOSARCINACEAE [AvL
(1984) 50 557567].
Autotrophic carbon dioxide fixation apparently occurs via
a pathway resembling that used for the synthesis of acetylCoA from carbon dioxide in ACETOGENESIS, although formyl
tetrahydrofolate synthase does not seem to be involved. AcetylCoA appears to be reductively carboxylated to pyruvate which
is converted to phosphoenolpyruvate (PEP); carboxylation of
PEP gives rise to oxaloacetate. Oxaloacetate appears to be
metabolized to 2-oxoglutarate as in the TCA cycle [see Appendix
II(a)] via citrate in Methanosarcina barkeri, via malate in
Methanobacterium thermoautotrophicum.
Some species (e.g. Methanococcus thermolithotrophicus,
Methanosarcina barkeri ) can carry out NITROGEN FIXATION
[Nature (1984) 312 284288; FEMS Ecol. (1985) 31 4755].
methanogenesis The biosynthesis of methane (CH4 ): an energyyielding process carried out by certain members of the domain
Archaea (METHANOGENS) in anaerobic environments that are
characterized by an Eh below about 330 mV (see e.g. ANAEROBIC DIGESTION, RUMEN and WETWOOD). Methane can be formed
from several substrates: carbon dioxide and hydrogen (or carbon dioxide and formate), acetate, methanol, or methylamines.
Methanogenesis involves a number of novel enzymes and coenzymes/cofactors [FEMS Reviews (1999) 23 1338].
Methane from carbon dioxide and hydrogen. Essentially, the
carbon atom of carbon dioxide is bound, sequentially, to
each of several C1 -carrier molecules and undergoes progressive
reduction (via formyl and methyl stages) to methane (see figure).
The final stage (reduction of CoM-S-CH3 ) is thermodynamically
0
favourable (1G0 greater than 100 kJ).
Methane from acetate. Growth on acetate is slower than that
on carbon dioxide and hydrogen; the free energy of the reaction
METHANOGENESIS. Two major pathways in the biosynthesis of methane: (i) synthesis from carbon dioxide, and (ii) synthesis from acetate.
(Methanol and methylamines are alternative substrates.) The final stage of biosynthesis, i.e. reduction of methyl-coenzyme M (see later), is
common to all the methane-forming pathways.
(i) Methane from carbon dioxide. In this pathway, the reduction of carbon dioxide can be linked to the oxidation of either hydrogen or
formate; the reactions shown occur in both hydrogen- and formate-oxidizing pathways.
Initially, carbon dioxide is reduced to a formyl residue on the coenzyme methanofuran (MFR; earlier name: carbon dioxide reduction factor,
CDR factor). Methanofuran is a long-chain molecule containing an aromatic ring and a terminal furan ring. This initial reduction is catalysed
by formylmethanofuran dehydrogenase. The formyl group is then transferred to tetrahydromethanopterin (THMP). Part of the THMP molecule
resembles FOLIC ACID, but the molecule is much larger than that of folic acid and it includes a sugar residue. The conversion of 5-formyl-THMP
to 5,10-methenyl-THMPC is catalysed by the enzyme N5 , N10 -methenyltetrahydromethanopterin cyclohydrolase.
Subsequent reductions in some methanogens (e.g. strains of Methanosarcina barkeri) involve an enzyme acting in association with coenzyme
F420 (factor 420), a 5-deazaflavin derivative that serves as an electron carrier. Strains of e.g. Methanococcus thermolithotrophicus use an
F420 -independent dehydrogenase to convert 5,10-methenyl-THMPC to 5,10-methylene-THMP.
Finally, the methyl group is transferred from THMP to coenzyme M (CoM-SH; 2-mercaptoethanesulphonic acid; HS(CH2 )2 SO3 ) in
preparation for its reduction to methane by the enzyme methyl-coenzyme M reductase; in all cases, the electron donor for this reduction is
coenzyme B (CoB; 7-mercaptoheptanoylthreonine phosphate). In the reductases from Methanobacterium thermoautotrophicum the active site
of the enzyme contains two molecules of coenzyme F430 (factor 430), a nickel-containing porphinoid.
Reduction of CoM-S-S-CoB regenerates the two coenzymes.
(ii) Methane from acetate. The sequence of reactions shown are those for Methanosarcina thermophila; the pathway differs slightly in some
methanogens. (Continued on page 470.)
469
Methanogenium
for the reduction of methyl groups from (three) other molecules
of methanol, the products being methane, carbon dioxide and
water. For methane synthesis, methyl groups must be bound
to coenzyme M in preparation for methanogenic reduction
involving CoB-SH (see figure). Contributing to this pathway
in Methanosarcina barkeri is an enzyme system that includes
methanol:corrinoid methyltransferase which catalyses the initial
transfer of methyl groups to the corrinoid moiety; further
enzymic activity transfers the methyl groups to CoM-SH.
In nature, methanogens are believed to produce most of the
methane from acetate; in vitro studies on the degradation of
rice straw in anoxic paddy soil have indeed shown that a high
proportion of methane is synthesized from acetate under those
conditions [FEMS Ecol. (2000) 31 153161]. Earlier work had
suggested that acetate may be the preferred substrate at 10 C,
with hydrogen being used at higher temperatures [FEMS Ecol.
(1997) 22 145153]. However, despite the overall picture, in
certain locations the contribution of hydrogen to methanogenesis
may be 70100% [FEMS Ecol. (1999) 28 193202].
The production of methane in anoxic soils can be suppressed
e.g. by nitrate; such inhibition appears to be due to the effects of
intermediates of the denitrification process [FEMS Ecol. (1999)
28 4961].
Methanogenium A genus of archaeans of the family METHANOMICROBIACEAE. Cells: cocci in which the cell wall consists
of an S LAYER only; the GRAM REACTION is negative. Species
include M. cariaci and M. marisnigri, both peritrichously flagellated organisms with an optimum growth temperature of ca.
20 C.
methanol utilization See METHYLOTROPHY.
Methanolobus A genus of METHANOGENS (see METHANOSARCINACEAE). The cells of M. tindarius are monoflagellated cocci
(ca. 1 m diam.); the cell wall consists of an S LAYER only.
Methanol and methylamine are methanogenic substrates. GC%:
ca. 46.
Methanomicrobiaceae A family of METHANOGENS (order METHANOMICROBIALES); genera: METHANOGENIUM, METHANOMICROBIUM,
METHANOSPIRILLUM.
Methanomicrobiales An order of METHANOGENS comprising the
families METHANOMICROBIACEAE, METHANOPLANACEAE and METHANOSARCINACEAE.
Methanomicrobium A genus of archaeans of the family METHANOMICROBIACEAE. Cells: typically short rods in which the cell
wall consists of an S LAYER only; the GRAM REACTION is negative.
M. mobile. Polarly flagellated rods which need e.g. acetate,
THIAMINE, PYRIDOXINE and PABA for growth. Habitat: RUMEN.
M. paynteri. Non-motile coccobacilli which occur in marine
sediments.
Methanoplanaceae A family of METHANOGENS (order METHANOMICROBIALES) [validation: IJSB (1984) 34 270]. One genus:
METHANOPLANUS.
Methanoplanus
A genus of archaeans of the family METHThe cells of M. limicola, the sole species, are
plate-like and are bounded by an S LAYER; this organism has
strong affinities with Methanogenium spp [Book ref. 157, p 17].
Methanosaeta A genus of obligately acetotrophic METHANOGENS
(methanogens which synthesize methane only from acetate). The
organisms, which include M. concilii and M. thermoacetophila,
are found e.g. in rice fields.
Methanosarcina
A genus of archaeans of the family METHANOSARCINACEAE. Cells: non-motile, coccoid to irregularly
shaped forms, ca. 13 m; the heteropolysaccharide-containing
cell wall is a thick (up to ca. 200 nm) layer which may
be laminated at the periphery. GAS VACUOLES are found in
some strains. The original type species, M. methanica, has been
rejected and replaced by M. barkeri [IJSB (1986) 36 492].
M. acetivorans. An acetotrophic marine species [AEM (1984)
47 971978].
M. barkeri. Cells grow as aggregates. Most strains can produce methane from carbon dioxide and hydrogen, acetate,
methanol or methylamine. Strain FR-19 lyses spontaneously in
substrate-depleted media [JGM (1985) 131 14811486].
M. mazei (cf. METHANOCOCCUS) is similar to M. barkeri but
differs e.g. in that M. mazei metabolizes acetate and methanol
readily but carbon dioxide and hydrogen poorly or not at all.
Methanosarcinaceae A family of METHANOGENS (order METHANOMICROBIALES). Depending on species or strain, some or
all of the following substrates are used for METHANOGENESIS: acetate, CO2 C H2 , methanol, methylamines. Genera:
METHANOSARCINA, METHANOTHRIX; it has been proposed that the
genera METHANOCOCCOIDES and METHANOLOBUS be incorporated
in the family [IJSB (1984) 34 444450].
Methanospirillum A genus of archaeans of the family METHANOMICROBIACEAE. M. hungatei is a facultative autotroph which
occurs in sewage sludge; the cells are curved, sheathed rods or
filaments that are lophotrichously flagellated.
Methanothermaceae A family of archaeans of the order
METHANOBACTERIALES. One genus: METHANOTHERMUS.
Methanothermus A genus of archaeans (family METHANOTHERMACEAE) in which the cell wall consists of two layers: a PSEUDOMUREIN-containing layer and an (outermost) S LAYER. Thermophilic (optimum: 83 C).
M. fervidus. Cells: non-motile rods, ca. 0.4 13 m; the
GRAM REACTION is positive. Methane is formed from carbon
dioxide and hydrogen but not from formate; yeast extract is
needed for growth. GC%: ca. 33.
Methanothrix A genus of archaeans of the family METHANOSARCINACEAE. M. soehngenii is common in anaerobic digestors; cells:
rods, ca. 0.8 2 m, or long, sheathed filaments each filament
often consisting of several hundred rods. The GRAM REACTION is
negative. Methane is formed from acetate but not from carbon
dioxide and hydrogen or from formate, methanol or methylamine.
ANOPLANACEAE.
METHANOGENESIS (continued)
Initially, acetate undergoes ATP-dependent activation to acetyl-CoA catalysed by the two enzymes acetate kinase and phosphotransacetylase. (In Methanosaeta, this section of the pathway differs in that the formation of acetyl-CoA is catalysed by acetate thiokinase.) The methyl
group is then transferred to tetrahydrosarcinapterin (THSP; analogous to THMP, above) by an enzyme complex that includes CO dehydrogenase
and CoA synthase; the activity of these enzymes results in the cleavage of carboncarbon and carbonsulphur bonds and also oxidation
of the carbonyl group (from acetyl-CoA) to carbon dioxide. Electrons derived from oxidation of the carbonyl group are involved in the final
methanogenic reduction of the methyl group after the latter has been transferred to coenzyme M.
In Methanosarcina thermophila the cam gene encodes a CARBONIC ANHYDRASE which apparently includes a signal peptide (see SIGNAL HYPOTHESIS);
it has been suggested that, by hydrating carbon dioxide in the periplasm, this enzyme may facilitate removal of carbon dioxide from the
cytoplasm and may thus promote conditions thermodynamically more favourable for methanogenesis.
470
methylene blue
MAP belongs to a diverse family of physiologically important
aminopeptidases [bacterial aminopeptidases: FEMS Reviews
(1996) 18 319344].
L-methionine biosynthesis See Appendix IV(d). (See also MICROCINS.)
methionine deformylase In bacteria: an enzyme which cleaves
the formyl group from methionine at the N-terminal of a newly
synthesized protein.
L-methionine-DL-sulphoximine See MSX.
methisazone See ISATIN-b-THIOSEMICARBAZONE.
Methocel See METHYLCELLULOSE.
methotrexate See FOLIC ACID ANTAGONIST.
methoxatin See QUINOPROTEIN.
methoxsalen 8-MethylPSORALEN.
methoxyamine (as a mutagen) See HYDROXYLAMINE.
6-methoxymellein A PHYTOALEXIN elicited from the carrot plant
e.g. by cupric or mercuric chloride.
methyl-accepting chemotaxis protein See CHEMOTAXIS.
methyl blue (cotton blue) A blue acid TRIPHENYLMETHANE DYE;
cf. LACTOPHENOL COTTON BLUE.
methyl bromide (CH3 Br) Methyl bromide vapour is fungicidal,
insecticidal and herbicidal; it has good powers of penetration
and is used as a fumigant.
methyl green A green basic TRIPHENYLMETHANE DYE. (See also
METHYL GREENPYRONIN STAIN.)
methyl greenpyronin stain (UnnaPappenheim stain) A stain
which can distinguish DNA (which stains green) from RNA
(which stains red); it can be used e.g. to distinguish lymphocytes
from (ribosome-rich) plasma cells.
methyl orange A PH INDICATOR: pH 3.04.4 (red to orangeyellow); pKa 3.6.
methyl red A PH INDICATOR: pH 4.46.2 (red to yellow); pKa
5.1.
methyl red test (MR test) An IMVIC TEST which determines the
ability of an organism to acidify a phosphate-buffered glucosepeptone medium to pH 4.4 or below. The medium is
inoculated and incubated for 48 h at 37 C or 5 days at 30 C.
Two drops of METHYL RED solution (0.02% w/v in ca. 50%
ethanol) are added to the culture; a red coloration indicates a
positive reaction. (N.B. Too short an incubation time may give a
false-positive reaction: some organisms (e.g. Klebsiella pneumoniae subsp. pneumoniae) initially form acidic metabolic products
which are later metabolized further.) The VOGESPROSKAUER TEST
can be performed after the MR test using the same culture.
methyl violet A composite TRIPHENYLMETHANE DYE which includes crystal violet and 4,40 -bis(dimethylamino)-400 -(methylamino)
triphenylmethyl chloride.
methyl viologen (Paraquat) 1,10 -Dimethyl-4,40 -dipyridinium, a
widely used herbicide. (See also PHOTOSYNTHESIS.) The reduced
form of methyl viologen is used e.g. as a reducing agent in
laboratory studies.
3-methyladenine-DNA glycosylase I See EXCISION REPAIR.
3-methyladenine-DNA glycosylase II See ADAPTIVE RESPONSE.
methylation (of DNA) See DNA METHYLATION.
methylcellulose (Methocel) An unbranched polymer (MWt ca.
143000) used e.g. to increase the viscosity of a medium in
order to slow down rapidly motile organisms see COUNTING
METHODS. (cf. FICOLL.)
methylcobalamin See VITAMIN B12 .
methylene blue A blue basic thiazine DYE used e.g. in STAINING and VITAL STAINING and as a redox indicator (E0 D
C11 mV at pH 7). (See also e.g. METHYLENE BLUE TEST; TOXOPLASMA DYE TEST.) Leuco methylene blue is the reduced (colourless) form of methylene blue. Loefflers methylene blue is
METHYLENE BLUE
metronidazole
occurring at 37 C; enrichment and primary isolation are
otherwise as described under METHYLOCOCCUS. A pink pellicle
is formed at 30 C; colonies are pink or yellow, consistently
pink on subculture. A blue diffusible pigment may be
formed in iron-deficient media. GC%: ca. 52. Type species:
M. methanica. (M. methanitrificans and M. methanooxidans
may be synonyms of Methylosinus trichosporium.)
Methylophaga
A proposed genus of marine methylotrophic
bacteria. The organisms are Gram-negative, strictly aerobic rods
which grow on methanol, methylamine(s) or fructose (but not
methane) and which require vitamin B12 ; those strains tested
use the RMP pathway for carbon assimilation. Two species:
M. marina, M. thalassia. [IJSB (1985) 35 131139.]
Methylophilus methylotrophus A species of obligately methylotrophic, non-methanotrophic bacteria (see METHYLOTROPHY)
which assimilate carbon via the RMP pathway and which have
been used in the production of SINGLE-CELL PROTEIN.
Methylosinus trichosporium A species of methanotrophic, obligately methylotrophic, typically rod-shaped or vibrioid bacteria
(see METHANOTROPHY, METHANE MONOOXYGENASE, METHYLOCOCCACEAE). [Effect of growth conditions on intracytoplasmic membranes and MMO activity: JGM (1981) 125 6384.]
methylotroph Any organism capable of METHYLOTROPHY.
methylotrophy Oxidative metabolism characterized by (i) obligate or facultative use of C1 COMPOUNDS as the sole source
of carbon and energy, and (ii) assimilation of formaldehyde
(produced during methylotrophic metabolism) as a major source
of carbon. Methylotrophy includes METHANOTROPHY.
Methylotrophic organisms include certain bacteria (e.g.
Hyphomicrobium, Methylobacterium spp, members of the
family METHYLOCOCCACEAE, Methylophaga spp, Methylophilus
methylotrophus, Microcyclus and Paracoccus denitrificans) and
some fungi (e.g. species of Candida, Hansenula and Pichia).
(cf. CARBOXYDOBACTERIA.)
(a) Methylotrophy in bacteria. Most of the C1 compounds
can be oxidized via a sequence of reactions which end in
HCHO ! HCOOH ! CO2 . Formaldehyde may be assimilated
by either the RMP PATHWAY or the SERINE PATHWAY, according
to species. (The serine pathway also assimilates some carbon
dioxide.) Energy may be derived from direct (non-cyclical)
oxidative pathways (e.g. methanol ! formaldehyde ! formate
! carbon dioxide) or from the (cyclical) RMP PATHWAY operating
in a dissimilatory mode. The TCA cycle appears to play little or
no part in the generation of energy from C1 substrates.
Methanol is used by most methylotrophs. It is oxidized
to formaldehyde by a QUINOPROTEIN: methanol dehydrogenase
(MDH; EC 1.1.99.8), whose electron acceptor is a soluble form
of cytochrome cL . [Roles for c cytochromes in methylotrophs:
JGM (1984) 130 33193325.]
Methane is oxidized to formaldehyde via methanol (see
METHANOTROPHY).
Methylamines are oxidized directly to formaldehyde in reactions that usually involve dehydrogenases or monooxygenases;
electrons from these substrates may be transferred to cyt b (via
a flavoprotein), or may be passed to cyt c via the blue protein
amicyanin.
The oxidation of formaldehyde to formate may be catalysed by various enzymes e.g. (i) MDH; (ii) NAD- and
reduced-glutathione-dependent formaldehyde dehydrogenase
(EC 1.2.1.1); or (iii) NAD(P)-independent non-specific aldehyde
dehydrogenase.
Formate is oxidized by NAD-dependent formate dehydrogenase (EC 1.2.1.2). (Some methylotrophs can use exogenous
formate as a source of energy and carbon.)
Metschnikowia
Mickle shaker An apparatus used e.g. for the ballistic disintegration of tissue or cells; in principle it resembles the BRAUN MSK
TISSUE DISINTEGRATOR. (See also BALLOTINI, CELL DISRUPTION and
ULTRASONICATION.)
miconazole (1-[2,4-dichloro-b-(2,4-dichlorobenzyloxyl)phenethylimidazole]) An AZOLE ANTIFUNGAL AGENT with a broad
spectrum of antifungal activity; it also has activity against certain bacteria (particularly Gram-positive species) and e.g. against
Naegleria fowleri. Miconazole is used mainly in the treatment of
superficial mycoses; it is usually administered topically, but can
be given intravenously (in cases of invasive or systemic mycosis)
or orally (e.g. to reduce intestinal populations of Candida spp).
Micrasterias A genus of placoderm DESMIDS.
microaerobic Refers to an environment in which oxygen is
present (cf. ANAEROBIC) but at a partial pressure which is (usually
significantly) lower than that in air.
microaerophilic Refers to any organism which grows optimally
in a MICROAEROBIC environment. (Frequently the term is also
used as a synonym of microaerobic.)
microalgae Microscopic algae particularly unicellular algae
such as CHLAMYDOMONAS, CHLORELLA, DIATOMS, etc.
microarray (DNA) See DNA CHIP.
Microascales An order of fungi of the ASCOMYCOTINA; the organisms are primarily saprotrophs in soil and dung, but some can
be pathogenic in man and other animals. Ascocarp: perithecioid or cleistothecioid, dark and solitary, sometimes setose;
hamathecium: absent. Asci: rounded, thin-walled, evanescent.
Ascospores: aseptate, pigmented. Genera: e.g. Microascus, PSEUDALLESCHERIA.
Microascus See MICROASCALES.
Microbacterium
A genus of catalase-positive, asporogenous
bacteria (order ACTINOMYCETALES, wall type VI see also PEPTIDOGLYCAN) which frequently occur in dairy products (e.g. spraydried milk, some cheeses) presumably as a result of improper
cleansing of dairy equipment. In culture the organisms are slender, pleomorphic, non-motile rods. Growth occurs optimally at
ca. 30 C on e.g. media containing yeast extract, peptone and
milk; L-(C)-lactic acid is formed from glucose. Some strains
produce a yellowish pigment. All strains grow aerobically. The
organisms are typically thermoduric, surviving e.g. 63 C/30 min
and 72 C/15 min. GC%: ca. 6970. Type species: M. lacticum.
(For M. thermosphactum see BROCHOTHRIX.)
microbe Syn. MICROORGANISM.
microbial insecticides See BIOLOGICAL CONTROL.
microbial leaching (of ores) See LEACHING.
microbial mat A complex, benthic microbial community which
forms a cohesive layer and which is typically dominated by
CYANOBACTERIA or other photosynthetic prokaryotes and occasionally e.g. by microalgae; microbial mats occur in those
regions where environmental stress tends to exclude, or reduce
the numbers of, metazoans e.g. in intertidal and hypersaline
regions, in hot springs, and around HYDROTHERMAL VENTS.
Microorganisms which occur in microbial mats include e.g.
species of Lyngbya and Microcoleus, various purple photosynthetic bacteria, Chloroflexus, and certain aerobic and anaerobic
chemotrophs, including SULPHATE-REDUCING BACTERIA.
Microbial mats are believed to have given rise to STROMATOLITES, and, under certain conditions, may have been precursor
material for KEROGEN and hydrocarbon deposits; in the latter context it has been suggested that oil is more likely to have been
derived from marine organic deposits than from terrestrial plant
material which, under appropriate conditions, gives rise to coal.
[Book ref. 154.]
microcomplement fixation
microbicidal Able to kill at least some types of microorganism.
(cf. MICROBISTATIC.)
microbiocoenosis A natural community of microorganisms (including algae, bacteria and protozoa) characterized by phases of
short-lived stability.
microbiological safety cabinet Syn. SAFETY CABINET.
microbiology The study of MICROORGANISMS and their interactions with other organisms and the environment (cf. CELLULAR
MICROBIOLOGY). There is considerable overlap between microbiology and certain other disciplines: e.g. biochemistry, immunology, molecular biology and PARASITOLOGY. Microbiology is also
directly relevant to certain aspects of medicine, veterinary science, agriculture, the food industry (see FOOD MICROBIOLOGY)
and various commercial processes (see INDUSTRIAL MICROBIOLOGY) as well as ecology and pollution studies (see e.g. CARBON
CYCLE, NITROGEN CYCLE, SULPHUR CYCLE, SEWAGE TREATMENT and
WATER SUPPLIES).
microbiota Microscopic organisms, particularly those in soil.
Microbispora A genus of bacteria (order ACTINOMYCETALES, wall
type III; group: maduromycetes) which occur e.g. in soil. The
organisms form branched aerial and substrate mycelium, the
former (commonly pink) giving rise to pairs of elongated spores;
when grown on certain solid media some species (e.g. M. parva)
deposit crystals of IODININ in the medium. The GC% of the type
species (M. rosea) has been reported to be ca. 74. [Ecology,
isolation and cultivation: Book ref. 46, pp. 21032117.]
microbistatic Able to inhibit the growth and reproduction of at
least some types of microorganism. (cf. MICROBICIDAL.)
microbody A particle, typically less than 1 m diam., consisting
of a collection of functionally related enzymes enclosed in a
membranous sac; microbodies occur in eukaryotic cells: see e.g.
GLYCOSOME, GLYOXYSOME, PEROXISOME. [Microbodies in urateutilizing yeasts: AvL (1985) 51 3343. How proteins get
into microbodies (review): BBA (1986) 866 179203.] (cf.
HYDROGENOSOME; LYSOSOME.)
microcapsule See CAPSULE.
microcarrier cell culture A system for culturing eukaryotic cells
in which the cells grow to form a confluent layer on the surface
of small solid particles suspended in a slowly agitated medium.
[Review: AAM (1986) 31 139179.] (See also TISSUE CULTURE.)
microcins A category of low-MWt BACTERIOCINS produced by
members of the Enterobacteriaceae and effective e.g. against
bacteria of the same family. The microcins differ from COLICINS
in their size, and also differ in that their synthesis is not induced
by conditions which trigger the SOS SYSTEM. Typically, microcins
are synthesized in the stationary phase, and synthesis tends to
be repressed in rich media.
The typical microcin ranges in size from a single modified
amino acid (microcin A15 appears to be a derivative of
methionine) to short or medium-sized peptides (up to 50
amino acid residues in length). Microcins are characteristically
thermostable (e.g. 100 C/30 min), soluble in methanolwater
(5:1), and resistant to extremes of pH and to certain proteases.
The microcins can be grouped according to their modes of
action: type A microcins inhibit certain metabolic pathways,
type B microcins inhibit DNA replication etc. For example, the
bacteriostatic microcin A15 inhibits homoserine succinyltransferase in the methionine biosynthetic pathway (see Appendix
IV(d)). The bactericidal microcin B17 inhibits DNA gyrase and
induces the SOS SYSTEM in Escherichia coli K12 [JGM (1986)
132 393402]. Microcin C7 is a heptapeptide which blocks
protein synthesis. (See also COLICIN V.)
Plasmids which specify microcins (M plasmids or, preferably,
Mcc plasmids) appear not to encode resistance to conventional
microconidium
microconidium (1) A SPERMATIUM. (2) A small CONIDIUM (cf.
MACROCONIDIUM).
microconjugant See CONJUGATION (1)(c).
microcycle sporulation Sporulation immediately following outgrowth of a spore. [Microcycle sporulation in Bacillus subtilis:
Book ref. 164, pp. 163167.]
microcyclic rusts Those rust fungi (see UREDINIOMYCETES) which
form only one type of binucleate spore, the teliospore i.e.,
aeciospores and uredospores are not formed; they include e.g.
some species of Puccinia.
Microcyclus
(1) A genus of fungi of the Dothideales. (2) A
genus of Gram-negative, obligately aerobic bacteria which occur
e.g. in soil and freshwater habitats. The cells are capsulated
curved rods, 0.31.0 1.03.0 m; one strain has a single polar
flagellum, but most strains are non-motile. The cells of some
strains contain GAS VACUOLES. The organisms grow chemoorganotrophically, but chemolithoautotrophic growth, with H2 as electron donor, has been reported for some strains; all strains tested
are facultative methylotrophs (see METHYLOTROPHY) which can
utilize e.g. formate and methanol. Catalase and oxidase Cve.
GC%: 6669. Type species: M. aquaticus. (Since the fungal
genus Microcyclus (Saccardo 1904) takes precedence, a new
name has been proposed for the bacterial genus: Ancylobacter
[IJSB (1983) 33 397398].) [Book ref. 22, pp. 133135.]
microcyst (1) (bacteriol.) A type of resting cell which may
or may not be resistant to heat, desiccation etc formed by
certain bacteria: e.g. Sporocytophaga and certain Nocardia
spp. (2) (bacteriol.) In the MYXOBACTERALES: syn. myxospore.
(3) (bacteriol.) Syn. coccoid body (see COCCOID BODIES). (4) In
some SLIME MOULDS: a resting structure formed by the rounding
up and encystment of an individual myxamoeba (cf. MACROCYST).
microcystin See MICROCYSTIS.
Microcystis
A phycological genus of unicellular blue-green
algae (CYANOBACTERIA) which may be referrable to SYNECHOCYSTIS. The cells are spherical, occur in mucilaginous
colonies, and contain GAS VACUOLES. Species are traditionally distinguished on the basis of cell size and colony form:
M. aeruginosa and M. flos-aquae form colonies in which numerous cells are embedded in a diffluent mucilage, while colonies
of M. marginata are surrounded by a distinct envelope. (Colony
form may be lost in culture.) The organisms do not fix nitrogen.
Microcystis spp are planktonic in fresh water, often forming
BLOOMS e.g. in reservoirs. Some strains of M. aeruginosa produce a cyclic peptide toxin, microcystin, which has hepatotoxic
effects in animals drinking the contaminated water; the toxin
appears to associate with cytoskeletal actin in a manner similar
to phalloidin (see PHALLOTOXINS). Another (peptide?) toxin (fast
death factor, microcystin-c) is a potent neurotoxin responsible
for convulsions, respiratory failure, and rapid death in animals.
microdilution broth test See DILUTION TEST.
Microellobosporia See STREPTOMYCES.
microfauna See MICROFLORA (2).
microfilament Any very thin filament particularly one of polymerized ACTIN.
microflora (1) In a microbiological context: the totality of
microorganisms normally associated with a given environment
or location (see e.g. BODY MICROFLORA); the term flora is often
used as an abbreviation in this context. (2) In a broader biological context: the microscopic plants and plant-like organisms
(e.g. bacteria, fungi, algae etc) normally present in a given environment or location, the term microfauna being used to refer
to the microscopic animals and animal-like organisms (e.g.
protozoa, nematodes) of that environment/location.
micropore
(ca. 5356) than that characteristic of the genus (7173). Many
species are cellulolytic. Some species produce useful antibiotics
(see e.g. GENTAMICIN). Type species: M. chalcea. [Book ref. 73,
pp. 6769.]
micron () 106 m (D MICROMETRE).
micronemes Small, convoluted, thread-like structures, oval or
circular in cross-section, which occur in members of the
APICOMPLEXA; function unknown.
micronucleus (ciliate protozool.) The smaller (commonly <5
m) of the two types of nucleus characteristically present in
ciliates (cf. MACRONUCLEUS); according to species a cell may
contain one, several or many micronuclei, although micronuclei
are absent in some viable strains of species which are normally
micronucleate. Micronuclei lack nucleoli, are characteristically
diploid, and their DNA (which occurs in chromosome form) is
transcriptionally inactive; they are involved in genetic recombination (see AUTOGAMY and CONJUGATION) and in the regeneration
of macronuclei.
microorganisms According to common usage: microscopic
organisms (and taxonomically related macroscopic organisms)
within the categories ALGAE, ARCHAEA, BACTERIA, FUNGI
(including LICHENS), PROTOZOA, VIRUSES and SUBVIRAL AGENTS.
Some authors do not regard viruses and subviral agents as
microorganisms reserving the term organism for an entity
which consists of one or more cells [Book ref. 159, pp. 1113];
other authors include PLASMIDS (as well as viruses) within the
category organisms [Book ref. 161, pp. 316].
micropalaeontology The study of microscopic fossils. (See also
FOSSIL MICROORGANISMS.)
microparticle enzyme immunoassay See LCR.
microperoxidase Part of a cytochrome c molecule (the haem
moiety together with part of the protein) which has peroxidase
activity and which is used e.g. in CHEMILUMINESCENCE studies.
microphotography Photography in which very small photographs are made of macroscopic or large objects. (cf. PHOTOMICROGRAPHY.)
microplasmodesmata Minute pores which occur in the septa in
certain filamentous prokaryotes: e.g. in hyphae of certain actinomycetes (see ACTINOMYCETALES) and in cyanobacterial TRICHOMES
(see also HETEROCYST).
Micropolyspora A (proposed) genus of bacteria (order ACTINOMYCETALES, wall type IV) which are found e.g. in mouldy
hay, compost and soil. The organisms form substrate and aerial
mycelium, both of which give rise to chains of spores; they
do not form mycolic acids. M. brevicatena, the former type
species of Micropolyspora, forms mycolic acids and has been
transferred to the genus Nocardia [JGM (1982) 128 503527],
leaving Micropolyspora a proposed genus nomen conservandum [Book ref. 73, pp. 123124]. [Proposal to conserve the
name Micropolyspora (with M. faeni as type species) and
new genus description: IJSB (1984) 34 505507.] M. faeni,
a common causal agent of FARMERS LUNG, forms substrate
mycelium of some shade of yellow, orange or brown, and a
white aerial mycelium. (M. faeni and M. rectivirgula appear
to be synonyms [JGM (1979) 115 343354].) M. viridinigra
and M. rubrobrunea have been transferred to the genus Excellospora.
Some authors use the name Faenia rectivirgula as a synonym
of M. faeni.
micropore (1) (formerly: micropyle, ultracytostome) In members
of the APICOMPLEXA: a small invagination of the pellicle (usually)
coincident with a discontinuity of the inner layer of the pellicle.
One or more micropores may be present in a given cell; they may
function as sites for the ingestion of food. (2) See GEOTRICHUM.
micropositioner
micropositioner See MICROMANIPULATION.
micropyle (1) In some species of coccidia (e.g. Eimeria stiedae):
a thin, polar region in the oocyst wall. (2) See MICROPORE (1).
microRNA (miRNA) See ANTISENSE RNA.
Microscilla See BACTERIA (taxonomy).
microscope slide Syn. SLIDE.
microscopy The use of an instrument (microscope) for examining
objects or details which are too small to be seen (or seen clearly)
MICROSCOPY. Figure 2. Image formation in bright-field microscopy, using a diffraction grating as a specimen. Light entering one slit of the
grating gives rise to zero-order rays (single arrowhead), first-order rays (double arrowhead) and second-order rays (terminally dashed lines).
An image is formed as a result of interference between diffracted and non-diffracted rays.
478
microscopy
MICROSCOPY. Figure 3. Amplitude and phase relationships in phase-contrast microscopy. (See text for explanation.)
MICROSCOPY. Figure 4. Image formation in phase-contrast microscopy: simplified diagrammatic scheme showing spatial relationships
between zero-order rays (solid lines from specimen to image plane) and first-order diffracted rays (dashed lines). (See text for explanation.)
image is further magnified by the eyepiece lens (see MAGNIFICAThe specimen is usually examined on a SLIDE which rests
on the stage. (See also HANGING DROP; MICROTOME; SMEAR; WET
MOUNT.)
For an image to be formed, light which has passed through
the specimen must differ from the background light in amplitude
(intensity) and/or in composition (e.g. colour); thus, an image
of the specimen is usually seen against a lighter (bright-field)
background. Some specimens are translucent and are therefore
poorly visible; such specimens can be made light-absorbing by
suitable STAINING.
Image formation is often depicted by ray diagrams. However,
for objects below a certain size, image formation can be described
satisfactorily only in terms of wave optics; this is because such
objects cause significant diffraction of light, and the formation
of an image depends on interference between diffracted and nondiffracted light waves. Image formation is shown in Fig. 2; the
KOHLER
ILLUMINATION). When using a HIGH-DRY OBJECTIVE, good
image formation also requires the use of a COVER-GLASS of
the correct thickness. (See also oil immersion objective under
RESOLVING POWER; cf. CONFOCAL SCANNING LIGHT MICROSCOPY.)
(b) Dark-field microscopy (dark-ground microscopy) is used
e.g. for examining objects too small to be seen by bright-field
microscopy. For low- or medium-power work, the underside of
TION).
479
microsome
the substage condenser is fitted with a central opaque disc (the
stop or patch stop) which allows only the peripheral rays to
pass through the condenser thus forming a hollow cone of
light whose apex is focused in the plane of the specimen; in the
absence of a specimen these rays diverge at such an angle that
none enters the objective so that the field of view appears dark
or black. (The NA of the condenser must be greater than that
of the objective.) A specimen scatters the rays, some of which
enter the objective and form a bright image of the specimen
against a dark background. For high-power work use is made of
a special oil-immersion condenser (e.g. a cardioid condenser)
within which the incident rays are twice reflected so that the
emergent rays form a hollow cone of large apical angle. (See
also RHEINBERG ILLUMINATION.)
(c) Phase-contrast microscopy. A colourless specimen which
absorbs little light (e.g. a non-pigmented living cell) is not
clearly visible by bright-field microscopy but may be seen
by phase-contrast microscopy. When such a specimen diffracts
light, the first-order waves are retarded by approximately 1/4wavelength (1/4l) and are of amplitude smaller than that of
the zero-order waves (Fig. 3(i)). If these zero-order and firstorder waves are allowed to interfere they will produce resultant
waves of amplitude (intensity) similar to that of the background
waves but differing from them in phase (Fig. 3(ii)); the phase
difference cannot be detected by the eye so that no image
is seen. (Background waves are waves which do not pass
through the specimen before entering the objective lens of the
microscope.) If, however, the zero-order and background waves
are first retarded by 1/4l (to eliminate the phase difference
between the first-order waves and the zero-order and background
waves), interference between zero-order and first-order waves
will produce a resultant wave (the image-forming wave) of
amplitude greater than that of the background wave (Fig. 3(iii)),
i.e., a visible image will be formed.
In a phase-contrast microscope the condenser has a ringshaped aperture in its front focal plane so that a hollow cone
of light can be focused (as a small bright ring) onto a phase
plate located in the back focal plane of the objective (Fig. 4).
The phase plate is a glass disc on which has been deposited
a ring of material (e.g. magnesium fluoride) of such thickness
that it retards by 1/4l the light it transmits. In the absence of
a specimen all the incident light is focused on and transmitted via the ring. When a specimen is examined, the zero-order
and background light is transmitted via the ring, but the firstand higher-order beams pass through the phase plate via regions
not located in the ring (Fig. 4). In the image plane, interference occurs between zero-order and diffracted light; the resultant
waves form a visible image because their amplitude is greater
than that of the background waves (Fig. 3(iii)). To increase
image contrast further the phase plate ring has deposited on it a
thin layer of light-absorbing material which decreases the amplitude of background and zero-order waves; thus the amplitude of
the image-forming wave becomes greater relative to that of the
background wave (Fig. 3(iv)). (The clarity of the image can be
improved by using a green filter in the microscope condenser.)
In the above scheme (negative or bright phase-contrast
microscopy) the zero-order beam is retarded by 1/4l, and
the specimen appears lighter than the background. In positive or dark phase-contrast microscopy the zero-order beam
is advanced 1/4l; the specimen appears darker than the background because destructive interference occurs between the zeroorder and first-order beams.
[Some improvements in phase-contrast microscopy: JM
(1983) 129 4962.]
(d) Interference-contrast microscopy (differential interference-contrast microscopy). This form of microscopy avoids
the haloes which surround images formed by phase-contrast
microscopy, and gives clearer images of fine detail. It can
detect minute differences in specimen thickness and/or refractivity such differences being indicated by colour differences
in the image. In microscopes based on the shear system (e.g.
the Nomarski microscope) light from the source is initially split
into two parallel beams. The object beam passes through the
specimen, while the reference beam passes through a clear or
relatively clear area of the slide; subsequently the beams interfere to form an image. In the double-focus system both beams
are co-axial the object beam being focused in the plane of the
specimen, and the reference beam being focused either above
or below this plane; subsequently, the beams interfere to form
an image.
(e) Fluorescence microscopy. In fluorescence microscopy a
(usually) FLUOROCHROME-treated specimen is irradiated with
ultraviolet radiation (or, in some cases, blue light) and the light
emitted (see FLUORESCENCE) forms the image of the specimen in
a manner similar in principle to that in bright-field microscopy.
(Some types of specimen exhibit autoFLUORESCENCE.) In a fluorescence microscope, the beam from a mercury-arc lamp, or a
tungsten lamp, is initially passed through an exciter filter which
transmits only the exciting radiation. The exciting radiation is
then focused onto the specimen either from below (transmittedlight fluorescence microscopy) or from above (incident-light
fluorescence microscopy, or epifluorescence microscopy). In epifluorescence microscopy exciting radiation enters the microscope
tube from the side and is reflected downwards, by a dichroic
mirror, through the objective onto the specimen; the imageforming light emitted from the specimen passes through the
objective, through the dichroic mirror (which does not reflect
light of visible wavelength), and through the eyepiece. In both
transmitted-light and epifluorescence microscopes, a barrier filter (D stopping filter) is placed below the eyepiece lens; this
transmits emitted light of longer wavelength but stops the
short wavelength exciting radiation thus protecting the eyes
and, in photomicrography, protecting the film against fogging.
One advantage of epifluorescence microscopy, compared with
transmitted-light fluorescence microscopy, is that the emitted
light is not partially absorbed within the thickness of the specimen; thus a brighter image can be obtained. (See also CITIFLUOR.)
(N.B. In all types of fluorescence microscopy it is necessary
to use non-fluorescent lenses, slides, cover-glasses, immersion
oil, etc.) (See also IMMUNOFLUORESCENCE; ACRIDINE ORANGE;
AURAMINERHODAMINE STAIN; CALCOFLUOR WHITE.)
(f) Ultraviolet microscopy is a form of microscopy in which
ultraviolet radiation is used both for illumination of the specimen
and for image formation; the image is recorded on a fluorescent
screen or on a photographic plate. Ultraviolet microscopy can
resolve finer detail than can bright-field microscopy because the
wavelength of the image-forming radiation is shorter than that
of visible light (see RESOLVING POWER).
(g) Epimicroscopy is any form of microscopy in which the
illuminating beam is focused on the specimen by the objective; in
this type of illumination (D vertical or incident-light illumination)
the objective acts simultaneously as the condenser and objective
lens. An example is epifluorescence microscopy: see (e) above.
microsome One of many small heterogeneous membranous vesicles obtained e.g. when eukaryotic cells are homogenized and
centrifuged; microsomes include e.g. vesicles formed from the
rough and smooth ENDOPLASMIC RETICULUM and from the CYTOPLASMIC MEMBRANE.
480
microtubules
microsource See BIOLUMINESCENCE.
Microsphaera See ERYSIPHALES.
Microspora A genus of filamentous, unbranched green algae
(division CHLOROPHYTA).
Microspora A phylum of PROTOZOA [JP (1980) 27 3758] which
are obligate intracellular parasites in a wide range of animals,
including vertebrates and invertebrates. Mitochondria are absent.
The organisms form spores which are small (commonly <10 m
diam.), unicellular in origin, and have walls which lack pores and
are not composed of valves (cf. MYXOZOA); each spore contains a
single uninucleate or binucleate sporoplasm (an amoeboid infective cell which is released on germination of the spore), and
a single tubular, coiled, extrusile polar filament which is not
enclosed within a polar capsule. A polar cap covers the attached
end of the tubular filament. In many species there is a membranous (vacuolar) region beneath the polar cap (the polaroplast or
polar sac). Classes: MICROSPOREA; RUDIMICROSPOREA. (See also
ENTEROCYTOZOON; cf. ASCETOSPORA.)
Microsporea A class of protozoa (phylum MICROSPORA) which
are parasitic in insects and other invertebrates, in poikilothermic vertebrates, and (rarely) in mammals. The microsporean
spore has (typically) a three-layered, dense, refractile wall, and
contains a single sporoplasm and a complex extrusion apparatus comprising the polar filament (which extends back from
the polar cap and coils around the inside of the spore wall)
and (typically) a polaroplast. When a spore is ingested by a
host animal, the polar filament is discharged explosively, everting to form a long tube; the explosive force is such that the
filament penetrates any host cell in its path, and the infective
sporoplasm can then pass through the filament and into the host
cell. [Role of pH-triggered Ca2C influx in the discharge mechanism: JCB (1985) 100 18341838.] The class contains two
orders: Minisporida (e.g. Burkea, Chytridiopsis, Hessea) and
Microsporida (e.g. Amblyospora, ENCEPHALITOZOON, GLUGEA,
NOSEMA, Pleistophora, THELOHANIA).
Microsporida See MICROSPOREA.
microsporidean (Pertaining to) a protozoon of the MICROSPORA
(formerly of the class Microsporidea, subphylum Cnidospora).
microsporidiosis Any disease caused by protozoa of the phylum
MICROSPORA. In man, infections occur in both immunocompetent
and immunocompromised individuals, although most isolations
appear to come from the latter group (particularly AIDS patients).
Infections may occur in any of various sites. For example,
travellers diarrhoea in immunocompetent hosts can be due
to intestinal infection by e.g. Encephalitozoon intestinalis or
Enterocytozoon bieneusi, while Encephalitozoon hellem, Nosema
ocularum and Vittaforma corneae have been isolated from the
eye. Species of Pleistophora infect skeletal muscle, while Trachipleistophora hominis infects skeletal muscle, eye, kidney and
nasopharynx. [Lab identification: JCM (2002) 40 18921901.]
In immunocompromised individuals, infection by microsporidia
is reported to be more common in patients with CD4C counts
below 100/l.
[Microsporidiosis: JMM (2000) 49 947967 (948952).]
Microsporum See DERMATOPHYTES.
microstome See TETRAHYMENA.
microstrainer See SEWAGE TREATMENT.
microsurgery See MICROMANIPULATION.
Microtetraspora A genus of bacteria (order ACTINOMYCETALES,
wall type III; group: maduromycetes) which occur e.g. in soil.
The organisms form a substrate mycelium (usually colourless,
grey, or yellowish) and aerial hyphae which give rise to spores
(typically) in chains of four. Type species: M. glauca. [Ecology,
isolation, cultivation: Book ref. 46, pp. 21032117.]
Microviridae
micrurgy Syn. MICROMANIPULATION.
Middelburg virus See ALPHAVIRUS.
middle T antigen See POLYOMAVIRUS.
Middlebrook 7H-9 broth A growth medium used for Mycobacterium spp; it contains mineral salts, pyridoxine hydrochloride,
biotin, sodium glutamate, sodium citrate, and either Tween 80
or glycerol. [Recipe: Book ref. 53, p. 1415.]
midland cattle disease A form of BOTULISM in cattle; the disease
is due to ingestion of forage or carrion contaminated with
C. botulinum type Cb (cf. FORAGE POISONING).
mid-point potential See REDOX POTENTIAL.
Mieschers tubes Sarcocysts in tissues (see SARCOCYSTIS).
MIF Migration inhibition factor: a CYTOKINE originally obtained
from specifically reactive T lymphocytes exposed to the relevant
antigen; in vitro, this factor is characterized by it ability to
inhibit the movement of macrophages away from the source
of MIF. (Other in vitro activities include the activation of NO
synthase (see NITRIC OXIDE) in macrophages.) MIF is associated
with DELAYED HYPERSENSITIVITY reactions and may account for
the accumulation and activity of macrophages in DH lesions.
The human MIF is a 12 kDa protein; its sources include
the pituitary gland. The precise in vivo role of MIF has not
been established; it may e.g. exert pro-inflammatory activity
as a counter-balance to raised levels of (anti-inflammatory)
glucocorticoids resulting from stimulation of the hypothalamicpituitaryadrenal axis.
migration inhibition factor See MIF.
mikamycins See STREPTOGRAMINS.
mildews (plant pathol.) See e.g. DOWNY MILDEWS and POWDERY
MILDEWS.
Miles and Misras method (drop method; drop plate method) A
COUNTING METHOD for determining the viable cell count of a
bacterial suspension. Serial dilutions (often log dilutions) of the
suspension are prepared. One drop (of known volume) from
each dilution is placed at a separate, recorded position on the
surface of a pre-dried agar PLATE; the drops are allowed to dry.
The plate is then incubated until visible colonies develop in the
small, circular areas corresponding to the drops. If a sufficient
number of dilutions has been prepared, a drop from one of
the dilutions will give rise to a countable number of discrete
colonies. Assuming that each viable cell in the drop gave rise
to a separate colony (and knowing the volume of the drop) the
viable count can be calculated. In practice, a count is calculated
from each of several drops on the plate, and the average is taken.
milfuram See PHENYLAMIDE ANTIFUNGAL AGENTS.
Milgo See ETHIRIMOL.
miliary Resembling millet seed. Miliary TUBERCULOSIS: a form
in which numerous small tubercles develop.
Miliolina See FORAMINIFERIDA.
milk (microbiological aspects) Milk consists primarily of water
containing proteins, soluble carbohydrates, electrolytes, lipids
and vitamins.
The major protein constituents of milk are CASEINS (which
occur in the form of complex micelles); there are also the socalled WHEY PROTEINS such as lactalbumin and lactoglobulin.
IMMUNOGLOBULINS occur in high concentrations in COLOSTRUM
and in relatively lower concentrations in milk. Various enzymes,
e.g., alkaline phosphatase (see PHOSPHATASE TEST), are normally
present in raw (i.e., untreated) milk. (See also LACTOFERRIN and
LACTOPEROXIDASETHIOCYANATEHYDROGEN PEROXIDE SYSTEM.)
The major carbohydrate, LACTOSE (ca. 50 g/l in cows milk),
contributes ca. 50% of the osmotic pressure of milk (which is
isotonic with blood plasma); small amounts of e.g. glucose and
galactose are also present.
Milton
microorganisms may contaminate (and survive within) milk
following collection.
(See also DAIRY PRODUCTS and MILK SPOILAGE.)
milk caps See LACTARIUS.
milk ring test (abortus Bang reaction/ringprobe; ABR) A test
for detecting BRUCELLOSIS in e.g. cattle. Milk from cows
infected with Brucella abortus contains antibodies to B. abortus
adsorbed to the fat globules. In the test, a small sample of milk
is mixed with a suspension of killed, stained cells of B. abortus,
shaken, and incubated for up to one hour. In a positive test
(antibodies present) the stained cells react with the antibodies
and are carried to the surface with the fat globules to form a
coloured layer (ring) of cream. In a negative test the cells
remain dispersed in the milk.
milk spoilage Souring (acidification) of milk (which often results
in clotting see CASEIN) can be caused e.g. by the growth of
Lactococcus lactis or other LACTIC ACID BACTERIA.
ROPINESS can be caused by slime-forming strains of Lactobacillus spp (e.g. L. brevis, L. casei ).
Broken cream (bitty cream), usually due to Bacillus cereus
or B. mycoides, is characterized by the development (in the
cream layer) of small particles which fail to emulsify on shaking;
it is thought to involve the activity of microbial LECITHINASES
on the milk fat globule membrane (see MILK) with consequent
coalescence of globules. Usually, the milk beneath a layer of
broken cream subsequently exhibits a non-acid clot (sweet
curdling) due to the effects of extracellular rennin-like microbial
enzymes on the milk CASEIN.
Malty off-flavours can be due e.g. to certain strains of
Lactococcus lactis which convert amino acids to aldehydes
(particularly leucine to 3-methylbutanal).
(See also LITMUS MILK and FOOD SPOILAGE.)
milk-vetch dwarf virus See LUTEOVIRUSES.
milkers nodule (milkers node) In man: non-ulcerating, red,
nodular (papular) lesions on the hands of milkers caused by
localized infection (via abrasions, cuts etc) with the PSEUDOCOWPOX virus.
milky disease An INSECT DISEASE affecting larvae of beetles of
the family Scarabaeidae. Originally, two forms of the disease
were recognized: type A, caused by Bacillus popilliae, and
type B, caused by B. lentimorbus (D B. popilliae var. lentimorbus); other species associated with milky disease e.g.
B. fribourgensis and B. euloomarahae may be varieties of
B. popilliae. Beetle larvae become infected when they ingest
spores of the pathogen; the spores germinate in the gut,
and the vegetative cells proliferate, subsequently invading the
haemolymph. Sporulation then occurs, resulting in ca. 5 109
spores/ml and giving the haemolymph the characteristic milky
appearance. B. popilliae, but not B. lentimorbus, forms a parasporal crystal similar to that of B. thuringiensis (see DELTAENDOTOXIN), but this apparently plays no role in milky disease.
The milky disease pathogens have been used successfully
in the USA for the BIOLOGICAL CONTROL of the soil-dwelling
larvae of the Japanese beetle (Popillia japonica); the spores
are produced commercially by the artificial inoculation of living
insect larvae. The pathogen may persist in suitable environments,
precluding the need for repeated application. B. popilliae cannot
grow at 37 C and is therefore unlikely to infect mammals.
millet red leaf virus See LUTEOVIRUSES.
millimicron (m) 103 (D NANOMETRE).
Millipore filter See FILTRATION.
Milstem See ETHIRIMOL.
Milton See HYPOCHLORITES.
min genes
A mixture of mini-Mu and helper Mu phages can function
more effectively in generalized TRANSDUCTION to rec C recipients than can Mu alone (which transduces only at very low
frequencies); this is probably due to the higher proportion of
phage particles containing significant amounts of bacterial DNA
which can undergo rec-dependent recombination with homologous regions of the recipients chromosome. However, if the
mini-Mu DNA has an intact A gene, recA recipients can be
used; in this type of transduction (termed mini-muduction) the
transduced DNA is integrated at random locations in the recipients chromosome, the inserted DNA being flanked by two
mini-Mu genomes in the same orientation.
(See also MUDLAC SYSTEM.)
mini-muduction See MINI-MU.
minimum haemagglutinating dose See MHD.
minimum haemolytic dose See MHD.
minimum inhibitory concentration (of an antibiotic) See MIC.
minimum lethal dose (MLD) (1) The minimum dose of a given
lethal agent sufficient to cause 100% mortality in a population
of test animals under given conditions.
(2) The minimum dose of a given lethal agent sufficient to
kill an individual of a given species of specified body weight
under given conditions.
Minisporida See MICROSPOREA.
Minitek system See MICROMETHODS.
mink Aleutian disease See ALEUTIAN DISEASE OF MINK.
mink cell focus-forming viruses See MCF VIRUSES.
mink enteritis virus See PARVOVIRUS.
mink leukaemia virus (MiLV) An endogenous type C retrovirus
(subfamily ONCOVIRINAE) isolated from the Mv-1-Lu mink lung
cell line. It is highly infectious for dog and donkey cells, weakly
infectious for mink cells, and non-infectious for murine, goat,
human and monkey cells. [Book ref. 114, pp. 118120.]
minocycline See TETRACYCLINES.
minor groove (in DNA) See DNA.
minus-progamone See PHEROMONE.
minus strand (of a gene) (mol. biol.) See CODING STRAND.
minus strand (virol.) See VIRUS.
minus 10 sequence See PROMOTER.
minus 35 sequence See PROMOTER.
minute virus of canines See CANINE PARVOVIRUS.
minute virus of mice See PARVOVIRUS.
minutes (in relation to genetic loci) See INTERRUPTED MATING
and MAP UNIT.
MIP channel A molecular pathway, consisting of a single protein in the cytoplasmic membrane (CM), which permits transmembrane movement of water and/or certain other uncharged
molecules. Such a channel (designated Aqp1) was first described
in the erythrocyte (red blood cell) membrane; it was later shown
to be analogous to the major intrinsic protein (MIP) in mammalian lens fibre, to the tonoplast intrinsic proteins in plants, and
to the GlpF protein in Escherichia coli. MIP proteins (found in
all classes of living organisms) share highly conserved regions.
A MIP channel consists of a single polypeptide which
apparently passes through the CM a number of times in a
series of loops; this structure is believed to form a pathway
for either water (channel D aquaporin) or glycerol (and/or
other uncharged molecules) (channel D glycerol facilitator ). (In
Lactococcus lactis the MIP channel transports both water and
glycerol.)
The aquaporin in E. coli (AqpZ) is encoded by gene aqpZ,
and the glycerol facilitator (GlpF) is encoded by gene glpF.
Mutants in aqpZ appear to grow poorly under low osmotic
mitochondrion
humans, some types of cancer have been linked to mutations
in genes homologous to mutS and mutL.)
Recent work suggests that asymmetry of ATPases on the MutS
dimer is crucial for mismatch repair and controls timing of the
repair cascade [EMBO (2003) 22 746756].
miso (soy paste; bean paste) A condiment made by fermenting
soybeans, usually mixed with cereal. A KOJI is prepared by
inoculating steamed rice with Aspergillus oryzae. Salt and
steamed soybeans are added, and the mixture is inoculated with
a starter culture of yeasts and bacteria (e.g. Zygosaccharomyces
rouxii, Pediococcus halophilus, Enterococcus faecalis), blended,
packed tightly into vats, and fermented at 2530 C for ca.
23 months. After ageing for ca. 2 weeks, the product is
blended, pasteurized and packaged, or freeze-dried and sold as
a powder. [Book ref. 5, pp. 3986.]
mis-sense mutation A MUTATION in which a codon specifying
one amino acid is altered so as to specify a different amino
acid. The effects of such a mutation range from none (a SILENT
MUTATION) to total inactivation of the gene product, depending
e.g. on the location of the amino acid in the product and on
the nature of the substituted amino acid relative to that of the
original. (cf. NONSENSE MUTATION; see also POINT MUTATION.)
MISTRESS Milk into steam treatment research equipment small
scale: equipment used for research into high-temperature (e.g.
UHT) methods of preservation in the food industry. Essentially,
milk is sprayed into a steam-containing vessel and, at the end
of the holding time, it is drawn through a hole into a vacuum
chamber where it cools by expansion.
mithramycin See CHROMOMYCIN.
mitochondrion A semi-autonomous intracellular organelle, one
or more (usually many) of which occur in most types of
eukaryotic cell (being absent e.g. in protozoa of the orders
Diplomonadida and Pelobiontida); RESPIRATION and the reactions
of the TCA CYCLE occur within the mitochondrion. Mitochondria
differ in size (<1 m to >10 m), shape, and number, according
to the type of cell in which they occur and to the physiological
state of that cell; a mitochondrion may be spherical, ovoid,
elongated, calyciform or irregularly shaped, and some are
branched.
Structure and composition. A mitochondrion consists of two
closed membranous sacs, one fitting closely within the other,
and an amorphous matrix (enclosed by the inner membrane)
which contains the mitochondrial DNA and enzymes of the
TCA cycle. The mitochondrial inner membrane is extensively
corrugated and forms plate-like, tubular, or finger-like structures
(cristae) which project into the matrix often more or less
perpendicular to the longitudinal axis of the mitochondrion;
the inner membrane contains components of the ELECTRON
TRANSPORT CHAIN, PROTON ATPASES and TRANSPORT SYSTEMS for
e.g. nucleotides, inorganic phosphate, and Ca2C . (See also ION
TRANSPORT.) The mitochondrial outer membrane contains PORINS
(see also VDAC).
Mitochondrial DNA (mtDNA) is typically in the form of
covalently closed circular, double-stranded molecules (differing
from the nuclear DNA e.g. in base composition and buoyant
density); mtDNA is linear in e.g. certain ciliates (including
Paramecium), Physarum polycephalum, and Hansenula mrakii.
Mitochondrial genes employ a GENETIC CODE (q.v.) which differs
in some respects from the universal code, and some fungal
mitochondrial genes contain introns (see SPLIT GENE). Genetic
recombination can occur between mtDNAs. (See also PETITE
MUTANT.)
mitogen
an intermediate and may bind DNA non-covalently and intercalatively (see INTERCALATING AGENT). Preferred sites for alkylation are the O-6 groups of guanine residues. (Reduced mitomycin
will also react with RNA and, to a lesser extent, protein.) Alkylation of B-DNA by mitomycin can cause conformational changes
that may involve the transition to Z-DNA. Mitomycin is a potent
inducer of lysogenic bacteriophages; viral DNA synthesis is relatively resistant to mitomycin.
mitoplast The inner membrane of a MITOCHONDRION together
with the mitochondrial matrix.
mitosis (karyokinesis) A sequence of events which culminates in
the division of a eukaryotic nucleus into two genetically similar
or identical nuclei whose ploidy is the same as that of the parent
nucleus; mitosis occurs during asexual (vegetative) cell division.
(cf. MEIOSIS.)
Different types of mitosis occur among the various types of
eukaryotic cell. The best-known (typical) form of mitosis is
that which occurs in the cells of higher animals and e.g. in
some protozoa; it involves the following stages (in chronological order).
Prophase. Individual CHROMOSOMES, each having previously
divided into two chromatids, condense and become visible
by light microscopy. The NUCLEOLUS becomes indistinct and
then invisible. MICROTUBULES of the CYTOSKELETON disassemble,
forming a pool of tubulin subunits. From each of two pairs of
CENTRIOLES (lying close to each other in the cytoplasm) arises
a radial array of microtubules (referred to as an aster ). Those
microtubules which extend from each centriole pair towards the
other elongate the centriole pairs concomitantly moving apart
until each eventually forms one pole of a bipolar microtubular
mitotic spindle; microtubules from each of the centriole pairs
(D polar microtubules or polar fibres) overlap in the mid-region
of the spindle.
Prometaphase. The nuclear membrane breaks into pieces.
KINETOCHORES develop on the chromosome centromeres, and
from each kinetochore kinetochore microtubules (D k-MTs;
kinetochore fibres) grow out more or less perpendicularly to the
long axis of the chromosome. The k-MTs apparently begin to
interact with the spindle (in some as yet unknown way) causing
the chromosomes to execute rapid movements.
Metaphase. The chromosomes become arranged in a layer (the
metaphase plate) midway between the poles of the spindle and
perpendicular to its axis. The metaphase plate may be maintained
for some time, each chromosome possibly being held in dynamic
equilibrium by equal and opposite forces generated within the
spindle.
Anaphase. The two chromatids of each chromosome appear
to move along stationary k-MTs to opposite poles of the
spindle; de-polymerization of the k-MTs apparently occurs at
the kinetochores the kinetochores possibly being involved in
generating the force needed to propel the chromatids towards
their respective poles [JCB (1987) 104 918]. As the k-MTs
shorten, the polar microtubules elongate and the spindle poles
move further apart.
Telophase. The chromatids become less clearly visible, and a
nuclear membrane assembles around each group of chromatids
to form two new nuclei in each of which a new nucleolus
appears. [Cell-free system for studying reassembly of the nuclear
envelope: Cell (1986) 44 639652.]
Telophase is followed by CYTOKINESIS. The non-dividing
nucleus is called the interphase nucleus; DNA replication occurs
during interphase.
In many microorganisms mitosis differs significantly from that
described above; thus, e.g. there are at least four distinct types of
MM virus
been reported e.g. for an iron-oxidizing bacterium [JGM (1984)
130 13371349] and for Alcaligenes eutrophus [JGM (1984)
130 19871994]. (See also CHEMOLITHOHETEROTROPH.)
Miyagawanella See CHLAMYDIA.
MK Menaquinone: see QUINONES.
MK broth MULLERKAUFFMANN
BROTH.
MK-0787 See THIENAMYCIN.
MLD MINIMUM LETHAL DOSE.
MLEE MULTILOCUS ENZYME ELECTROPHORESIS.
MLOs Mycoplasma-like organisms: wall-less, non-helical, prokaryotic organisms which are associated with invertebrates and
plants and which are the causal agents of a number of plant
YELLOWS diseases. MLOs have not been cultured in vitro and
have not been formally classified, although they are usually
associated, taxonomically, with the MOLLICUTES. Various MLOs
have been shown to lack a Spiroplasma-specific antigen [JGM
(1983) 129 19591964]. [Book ref. 22, pp. 792793; wall-less
prokaryotes and plants: ARPpath. (1984) 22 361396.]
From the mid-1990s, MLOs were referred to by the trivial
name phytoplasma. Individual MLOs are now being called by
names such as Candidatus Phytoplasma australiense.
[Phytoplasma: ARM (2000) 54 221255.]
MLR (immunol.) Mixed lymphocyte reaction (D mixed leucocyte reaction or mixed leukocyte reaction): mutual interaction,
with blast transformation and proliferation of T cells, which
occurs when leukocytes from two allogeneic individuals are
mixed and cultured; the greater the disparity between antigens
(e.g. MHC class II antigens) on donor and recipient cells the
greater the degree of proliferation. (The degree of proliferation
may be assessed e.g. by measuring the amount of radioactive
thymidine (a DNA precursor) taken up by the cells.)
MLR (which takes several days to perform) is used e.g. to
assess the compatibility of transplant donors and recipients. A
negative reaction (no proliferation of T cells) is given when cells
are derived from identical twins.
MLS antibiotics Macrolide, lincosamide and streptogramin Btype antibiotics: a group of structurally distinct antibiotics all of
which act on the 50S subunit of 70S ribosomes (see MACROLIDE
ANTIBIOTICS, LINCOSAMIDES and STREPTOGRAMINS). [Symposium
on MLS antibiotics: JAC (1985) 16 (supplement A).]
Co-resistance to MLS antibiotics in staphylococci, streptococci and streptomycetes can be due to N 6 -methylation of adenine residues in 23S rRNA (see STREPTOGRAMINS).
Strains of Streptococcus pyogenes and S. pneumoniae that
express the M phenotype contain a macrolide-efflux mechanism which confers resistance to macrolides concomitant with
sensitivity to lincosamides and B streptogramins (see MACROLIDE
ANTIBIOTICS).
MLSB=c strains See STREPTOGRAMINS.
MLST (multilocus sequence typing) A method for TYPING
pathogenic bacteria which permits long-term, global-scale
tracking of virulent and antibiotic-resistant strains, with
information made available on the Internet. In MLST, strains are
characterized and classified on the basis of nucleotide sequences
in specific alleles, this approach giving rise to categorization
which is apparently stable over long periods of time.
[MLST (review): TIM (1999) 12 482487. MLST of
methicillin-resistant and methicillin-sensitive clones of Staphylococcus aureus: JCM (2000) 38 10081015.]
MluI See RESTRICTION ENDONUCLEASE (table).
MLV MURINE LEUKAEMIA VIRUS.
MM MINIMAL MEDIUM.
MM virus See CARDIOVIRUS.
Monilia
Moniliales
monocins See BACTERIOCIN.
monocistronic mRNA See MRNA.
monoclonal antibodies A population of identical antibodies
(see ANTIBODY), all of which recognize the same specific
DETERMINANT on a simple or complex antigen or hapten. (cf.
POLYCLONAL ANTISERUM.) A given population of monoclonal
antibodies may be able to react with each of two apparently
unrelated antigens if, by chance, those antigens happen to share
a common determinant; thus, e.g., monoclonal antibodies which
combine with a particular mouse myeloma protein can combine
with human C-reactive protein. (cf. CROSS-REACTING ANTIBODY.)
Monoclonal antibodies are obtained from B-cell HYBRIDOMAS.
Monoclonal antibodies have an enormous range of actual or
potential uses. These include e.g. characterization and detection
of viruses [e.g. plant viruses: MS (1984) 1 7378] and other
microorganisms; tissue typing; the study of changes in cellsurface antigens on lymphoid cells during maturation; and the
preparation of IMMUNOTOXINS.
monocystid gregarine Syn. acephaline gregarine.
Monocystis A genus of protozoa (subclass GREGARINASINA) many
species of which are parasitic in the earthworm (Lumbricus spp).
Sporozoites enter the seminal vesicles. The developing parasites
(trophozoites) occur intracellularly in the sperm morulae; the
fully-grown, extracellular acephaline trophozoites (gametocytes)
associate in pairs (syzygy) and each pair forms a gametocyst
within which many gametes develop. The gametes fuse in pairs,
and each zygote forms a cyst (sporocyst, pseudonavicella) within
which 8 sporozoites develop.
monocyte A large (diam. 1020 m) phagocytic LEUCOCYTE
which contains a single, large, spherical or indented nucleus,
and azurophilic peroxidase-containing granules; ca. 200800
monocytes/ml occur in normal adult human blood. Monocytes
differentiate to become MACROPHAGES. Suspensions of monocytes may be prepared e.g. by density flotation [JIM (1984) 69
7177] or by the use of Sephadex [JIM (1984) 71 2536].
monocytosis Syn. MONONUCLEOSIS.
Monod equation See SPECIFIC GROWTH RATE.
Monodictys See HYPHOMYCETES; see also SOFT ROT (sense 1).
monoecious Refers to an organism in which the male and
female reproductive structures occur in the same individual. (cf.
DIOECIOUS.)
monogeneric Refers to a taxon which has only one genus.
monogenic mRNA See MRNA.
monokaryotic Having one nucleus per cell.
monokines Certain soluble, biologically active products of
MACROPHAGES e.g. INTERLEUKIN-1.
monolayer culture See TISSUE CULTURE.
Monomastix See MICROMONADOPHYCEAE.
monomitic See HYPHA.
monomorphic Refers to an organism which occurs in only one
form or MORPHOTYPE. (cf. POLYMORPHISM.)
Mononegavirales A taxon containing viruses which have nonsegmented, negative-sense ssRNA genomes, including members
of the FILOVIRIDAE, PARAMYXOVIRIDAE and RHABDOVIRIDAE and
(probably) the BORNA DISEASE VIRUS.
mononuclear leucocyte (mononuclear phagocyte) (1) Syn. MACROPHAGE. (2) Syn. MONOCYTE. (3) A macrophage or monocyte.
mononuclear phagocyte See MONONUCLEAR LEUCOCYTE.
mononucleosis (monocytosis) The condition in which increased
numbers of monocytes are present in the blood. (cf. INFECTIOUS
MONONUCLEOSIS.)
monooxygenase (hydroxylase; mixed-function oxidase; mixedfunction oxygenase) An OXYGENASE (EC 1.13.12) which catalyses the incorporation of one atom of molecular oxygen into
Morbillivirus
an appropriate liquid medium and incubated. The Moore-swab
technique appears to be more effective in small sewers [AEM
(1986) 51 425426].
Moorella See CLOSTRIDIUM.
Mopeia virus See ARENAVIRIDAE.
MoraxAxenfeld bacillus See MORAXELLA.
Moraxella A genus of oxidase Cve, typically catalase Cve Gram
type-negative bacteria of the family MORAXELLACEAE which
occur on mucous membranes (e.g. respiratory tract) in man and
other mammals; strains of Moraxella can act as opportunist
pathogens.
Cells: short rods/cocci which may occur singly or in
pairs; non-motile, but may exhibit TWITCHING MOTILITY. Nonpigmented.
Some moraxellae are nutritionally fastidious; all strains can
grow on blood agar (some better on chocolate agar); many
strains are able to grow on rich, non-blood-containing media
or even nutrient agar. Acid is not produced from carbohydrates. Nitrate is reduced by some strains. Optimum growth
temperature: 3336 C. Unlike species of Neisseria, no strain
produces CARBONIC ANHYDRASE. GC%: 4047.5. Type species:
M. lacunata.
Species include:
M. atlantae. Non-haemolytic. Serum is needed for growth;
coagulated serum is not liquefied. Growth is stimulated by bile
salts. Nitrate is not reduced.
M. bovis. A causal agent of e.g. INFECTIOUS KERATITIS. Some
strains are catalase ve. Usually haemolytic (on human blood).
Coagulated serum is usually liquefied. Nitrate is usually not
reduced. Acetate, butyrate, ethanol and lactate can be metabolized in complex media.
M. lacunata (the MoraxAxenfeld bacillus). A causal agent
of CONJUNCTIVITIS. Non-haemolytic on human blood. Serum is
required for growth; coagulated serum is liquefied. Nitrate is
reduced. Phenylalanine deaminase and urease are not formed.
Acetate, butyrate and lactate can be metabolized in complex
media.
M. catarrhalis (formerly Branhamella catarrhalis). A causal
agent of e.g. respiratory tract infections, acute OTITIS MEDIA and
SINUSITIS. Non-haemolytic. Many strains can grow on nutrient
agar. On blood agar, the colonies are whitish, convex, and 12
mm in diam. after 24 hours. Most strains reduce nitrate and
nitrite, and most or all strains are reported to produce a DNase.
[Review: Drugs (1986) 31 (supplement 3) 1142.]
M. caviae, M. cuniculi and M. ovis have been regarded
as members of a subgenus, Branhamella, within the genus
Moraxella or as species incertae sedis within the genus Neisseria (so-called false neisseriae) [Book ref. 22, pp 290296].
Moraxellaceae A family of Gram type-negative bacteria comprising the genera ACINETOBACTER, MORAXELLA and PSYCHROBACTER [IJSB (1991) 41 310319].
morbidity (1) The state or condition of being diseased. (2)
(morbidity rate) The number of cases of a given disease in
relation to the overall population (quoted e.g. as cases per
100000 or per million per annum). (cf. MORTALITY RATE.)
morbilli Syn. MEASLES.
morbilliform Resembling measles.
Morbillivirus (measlesrinderpestdistemper (MRD) virus group)
A genus of viruses of the PARAMYXOVIRIDAE in which the virions have haemagglutinin but no neuraminidase activity. Virions
contain proteins N (nucleocapsid), P (nucleocapsid-associated
phosphorylated), H (haemagglutinin), F (fusion) and M (membrane or matrix). (cf. PARAMYXOVIRUS.) All members share a
Morchella
Mortierellaceae See MUCORALES.
mos
An ONCOGENE first identified as the transforming determinant of MOLONEY MURINE SARCOMA VIRUS (Mo-MSV). The
c-mos sequences are hypermethylated, apparently transcriptionally silent (or expressed at very low levels) in normal and
transformed murine cells, and lack introns. Wild-type Mo-MSV
expresses v-mos only at very low levels in cell culture, but a
temperature-sensitive mutant (ts110) produces higher levels of
an unstable gag-mos fusion protein (MWt ca. 85000) which has
serine or threonine protein kinase activity [review: JGV (1985)
66 18451853]. [Properties of mouse and human c-mos loci:
Book ref. 113, pp. 281289.]
mosaic (plant pathol.) A form of leaf VARIEGATION in which two
or more colours, or shades of colour, develop the differently
coloured areas being somewhat angular with relatively sharp,
clear-cut boundaries between them. (cf. MOTTLE.) Mosaics occur
in plants infected systemically with certain PLANT VIRUSES;
however, similar leaf patterns may be an inherited characteristic
or may result from the effects of toxins produced by leaf-feeding
arthropods.
mosquito iridescent virus See CHLORIRIDOVIRUS.
moss starch Syn. LICHENIN.
most probable number method See MULTIPLE-TUBE METHOD.
motB gene See FLAGELLUM (a).
motile (microbiol.) Capable of MOTILITY.
motile colonies (1) (bacteriol.) The colonies of certain bacteria,
e.g. Bacillus circulans, can migrate across the surface of a culture
plate; the track of such movement is often marked by lines
of bacterial growth which arise from cells left behind by the
migrating colony.
(2) (algol.) See e.g. SYNURA and VOLVOX.
motility (microbiol.) Locomotion, i.e. an active process in which
a cell or organism moves from place to place by expending
energy to exert force(s) against the surrounding medium or the
contiguous substratum; passive movements due to changes in
buoyancy (see e.g. GAS VACUOLE) are not regarded as true motility
(see also TWITCHING MOTILITY).
Not all microorganisms are motile, i.e. capable of exhibiting
motility; however, those which are motile occur among the
algae, archaeans, bacteria, fungi and protozoa. Some nonmotile organisms have motile stages in their life cycles e.g.
propagules, gametes.
Motility is an advantage because it enables an organism
to respond e.g. to certain environmental stimuli. (See also
CHEMOTAXIS.)
Locomotion may be achieved in various ways, depending on
organism.
(a) Amoeboid movement is characteristic e.g. of some sarcodines (see PSEUDOPODIUM).
(b) CILIUM-mediated locomotion occurs in members of the
CILIOPHORA (see also METACHRONAL WAVES).
(c) Euglenoid movement: see EUGLENA.
(d) FLAGELLAR MOTILITY involves the activity of one or more
flagella (or periplasmic flagella in the SPIROCHAETALES) and is
found in many bacteria, protozoa (see MASTIGOPHORA) and algae,
and in some fungi (limited to certain lower fungi e.g. the
zoospores of chytrids).
(e) GLIDING MOTILITY occurs in some prokaryotes (e.g. Beggiatoa, Oscillatoria), and e.g. in some diatoms and desmids.
[The motility apparatus in shock-frozen gliding cells of Myxococcus xanthus (electron micrographs): Microbiology (2001)
147 939947.]
(f) Gregarine movement, which occurs in some gregarines, is
apparently similar or identical to GLIDING MOTILITY (q.v.).
mRNA
predisposition, hormonal status, number of pregnancies, etc.
A critical factor in tumorigenesis is believed to involve the
insertion of the provirus at particular sites in the mouse genome;
two such sites have been implicated (int-1 and int-2), neither
of which shows homology with any known cellular or viral
ONCOGENE. Integration of an MMTV provirus near one of
these loci appears to activate the expression of a host gene
which is normally silent, possibly by exerting an enhancer
function. [Reviews of oncogenesis by MMTV: Book ref. 110,
pp. 175195; JGV (1985) 66 931943.]
mouse poliomyelitis See THEILERS MURINE ENCEPHALOMYELITIS
VIRUS.
mousepox See ECTROMELIA VIRUS.
mouth fungus (in fish) See COLUMNARIS DISEASE.
mouth microflora The microflora of the human mouth may
include e.g. species of ACTINOMYCES, BACTEROIDES, CAMPYLOBACTER, CAPNOCYTOPHAGA, EIKENELLA, FUSOBACTERIUM, LEPTOTRICHIA, ROTHIA, SELENOMONAS, STAPHYLOCOCCUS, STREPTOCOCCUS, TREPONEMA, WOLINELLA, VEILLONELLA, and various
yeasts (e.g. Candida albicans) and protozoa (e.g. Entamoeba
gingivalis and Trichomonas tenax ). Some of these organisms
occur primarily in microaerobic or anaerobic microenvironments
such as the gingival sulcus. (See also BODY MICROFLORA; DENTAL PLAQUE; GASTROINTESTINAL TRACT FLORA; RESPIRATORY TRACT
MICROFLORA; STOMATITIS.)
moving-boundary electrophoresis See ELECTROPHORESIS.
moxalactam (latamoxef) An OXACEPHEM antibiotic which is
active against a wide range of Gram-negative bacteria.
moxifloxacin A QUINOLONE ANTIBIOTIC (q.v.).
Mozambique virus See ARENAVIRIDAE.
mozzarella cheese See CHEESE-MAKING.
MPa 106 PASCAL.
MPEDn In a heat STERILIZATION process: the most probable
effective dose of thermal energy required to achieve an n-log10
reduction in the numbers of a given microbial contaminant.
mpl gene See PEPTIDOGLYCAN.
MPN method See MULTIPLE-TUBE METHOD.
MppA See PEPTIDOGLYCAN.
MPT64 See ESAT-6.
Mr RELATIVE MOLECULAR MASS.
MR test See METHYL RED TEST.
MR vaccine Measlesrubella vaccine.
Mrad 106 rad (see RAD).
mrcA gene See PENICILLIN-BINDING PROTEINS.
mrcB gene See PENICILLIN-BINDING PROTEINS.
MRD virus group See MORBILLIVIRUS.
MreB protein See CELL CYCLE (b) (determination of shape).
MRHA Mannose-resistant haemagglutination (see FIMBRIAE).
mRNA Messenger RNA: any RNA molecule which functions as
a template for the assembly of amino acids during PROTEIN
SYNTHESIS (see GENETIC CODE). In all cells, and in DNA viruses,
the mRNA is transcribed from DNA (see TRANSCRIPTION); in
RNA viruses, the genome may or may not be able to function
directly as mRNA (see VIRUS).
(a) Prokaryotic mRNAs. Many bacterial mRNAs are functional as primary transcripts, i.e. they do not require posttranscriptional maturation. An mRNA molecule may contain the
transcript of a single gene (monocistronic or monogenic mRNA)
or, more commonly, transcripts of two or more genes (polycistronic or polygenic mRNA). (See also OPERON.)
A polycistronic mRNA contains several distinct regions: a
50 LEADER; coding regions (structural gene transcripts), each
beginning with a translation initiation codon and consisting of a
493
mRNA
linear sequence of codons; and sometimes a 30 -terminal trailer.
The coding regions may or may not be separated by non-coding
intercistronic regions (see also OVERLAPPING GENES).
The synthesis, translation and degradation of bacterial mRNA
are closely linked phenomena; typically, bacterial mRNAs have
a very short half-life, and in some cases degradation may
begin even before transcription has been completed. mRNA is
particularly prone to degradation in the absence of translation:
see POLAR MUTATION. (cf. RRNA.) (See also S LAYER.)
The secondary structure of bacterial mRNA may be important
in determining its stability. Stable mRNAs typically contain
multiple secondary structures, particularly in the 30 -terminal
region, and these may serve to protect the molecule from 30 to-50 processive exonucleases present in the cell. (One function
of the GC-rich stem-and-loop structure in a rho-independent
terminator see TRANSCRIPTION may be to protect the 30 end
of the transcript from degradation by exonucleases.) (See also
RETROREGULATION.)
Some bacterial mRNAs e.g. that transcribed from the
Escherichia coli gene lpp (which encodes an outer membrane
lipoprotein) have atypically long half-lives. Moreover, the rate
of degradation of mRNAs can be affected by growth conditions.
For example, in E. coli the half-life of at least some mRNAs is
greatly extended during slow anaerobic growth (doubling time:
700 minutes); in these conditions the rate of synthesis of mRNA
is much lower, so that extended half-life may be a mechanism
for maintaining the expression of such genes during anaerobiosis
[Mol. Microbiol. (1993) 9 375381].
In Escherichia coli, no known exonuclease can degrade RNA
in the 50 -to-30 direction (i.e. in the direction of transcription and
translation). mRNA degradation appears to involve the activity
of endonuclease(s) and (30 -to-50 ) exonuclease(s) (e.g. RNASE II);
small pieces of RNA (10 nucleotides in length) are apparently
degraded to single nucleotides by an enzyme designated RNase
[JB (1991) 173 46534659].
Polyadenylation. Many prokaryotic mRNAs have a short (e.g.
1050 nt) polyadenylate tail at the 30 end. This poly(A) (AA-A. . .) tail, whose synthesis involves a poly(A)polymerase,
may influence the half-life (stability) of those mRNAs whose
30 terminus contains a stemloop structure encoded by a rhoindependent transcription terminator; such 30 stemloop structures tend to resist enzymic degradation, and polyadenylation
may facilitate degradation by providing a suitable binding site
for enzymes such as 30 -exonuclease polynucleotide phosphorylase.
Interestingly, mutations in gene pcnB which encodes the
Escherichia coli poly(A)polymerase I (PAP I) can reduce
the copy number of plasmid ColE1. Apparently, the plasmidencoded antisense molecule RNA I (which inhibits RNA II) is
normally polyadenylated, polyadenylation assisting degradation
of the molecule; the absence of polyadenylation in pcnB mutants
tends to stabilize RNA I, i.e. to enhance its inhibitory action on
RNA II causing inhibition of plasmid replication and, hence,
a reduction in copy number.
A poly(A) tail of 10 nucleotides was reported earlier in the
archaean Methanococcus vannielii [JB (1985) 162 909917.]
The poly(A) tail facilitates isolation of mRNAs by affinity
chromatography; thus, mRNAs can be isolated by exploiting
base-pairing specificity between the A-A-A. . . of mRNAs and
the T-T-T. . . of oligo(dT)-cellulose in the matrix. Isolation of
mRNAs can also be achieved e.g. by the use of DYNABEADS
coated with oligo-dT.
[Polyadenylation of mRNA in bacteria (review): Microbiology (1996) 142 31253133. Characterization of Escherichia coli
poly(A)polymerase: NAR (2000) 28 11391144. Polyadenylation in mycobacteria: Microbiology (2000) 146 633638.]
Introns. As in typical eukaryotic genes, some bacterial,
archaean and phage genes include introns (see SPLIT GENE).
In the transcripts of such genes any part corresponding to
an intron must be removed in order to produce a mature
mRNA that correctly encodes the gene product. Bacterial introns
are autocatalytic, i.e. enzymic activity that develops within a
correctly folded mRNA molecule automatically splices out the
relevant sequence of nucleotides. In at least some cases, splicing
may occur even while the nascent transcript is bound to the
ribosome, the ribosome pausing during excision of the intron
sequence. [Splicing and translation in bacteria: GD (1998) 12
12431247.]
(b) Eukaryotic mRNAs. In eukaryotes mRNA is synthesized
(by RNA POLYMERASE II) in the nucleus and must be exported to
the cytoplasm for translation; typically, mRNA is synthesized
as a large precursor molecule (pre-mRNA) which undergoes an
extensive maturation process involving capping at the 50 end
(see below), polyadenylation of the 30 end, and (commonly)
splicing out of introns (see SPLIT GENE). The mature mRNA
molecule is typically functionally monocistronic. (cf. POLYPROTEIN; see also SUBGENOMIC MRNA.)
Some eukaryotic genes are atypical in that they do not contain
introns thus obviating the need for splicing of mRNA; such
genes include most or all of those encoding histones as well as
e.g. the gene encoding interferon-b.
In the cytoplasm, mRNAs are relatively stable, and they
occur complexed with proteins to form messenger ribonucleoproteins, mRNPs (D informosomes). [Review: TIBS (1985)
10 162165.]
Polyadenylation. Most eukaryotic mRNAs have a poly(A)
(polyadenylate) sequence about 200 adenylate residues at
the 30 end. This poly(A) tail is not added to the complete transcript: at the end of transcription an endonuclease cuts the transcript at a specific site 1030 nucleotides downstream of an
AAUAAA (or similar) sequence thus creating an appropriate
30 terminus from which another enzyme, poly(A)polymerase, can
synthesize the polyadenylate tail. The function of the poly(A) tail
is unknown.
Some eukaryotic mRNAs do not have a poly(A) tail; for
example most or all mRNAs that encode histones are apparently
poly(A) .
Capping. Almost all eukaryotic mRNAs are modified (capped )
at the 50 end. Capping occurs shortly after the beginning of
transcription: an enzyme (guanylyl transferase) adds to the newly
formed 50 end of the molecule an inverted guanosine residue,
i.e. a guanosine residue linked 50 -to-50 to the 50 -triphosphate end
of the growing pre-mRNA molecule. A methyl group is then
transferred (by a specific 7-methyltransferase) to the N7 position
of the G cap to form the characteristic cap structure:
0
m7 G5 ppp5 N3 p5 N3 p . . .
A cap methylated only at this position is said to be of type 0.
0
Type 1 caps have an additional methyl group at the O2 -position
of the next (2nd) nucleotide, and sometimes also at the N6 position of a penultimate adenine residue; type 2 caps contain,
in addition to the type 1 methyl group(s), a methyl group at
0
the O2 -position of the 3rd nucleotide. Apparently, unicellular
eukaryotes contain only type 0 caps; type 1 caps predominate in
other eukaryotes.
The 50 cap enhances translation by promoting the formation of
the translation initiation complex; the recognition of the cap by
494
muciferous body
culture media typically contain 4% NaCl and they are incubated
at e.g. 3035 C. MRSA grows in 2448 hours when inoculated (104 cfu) onto MuellerHinton agar containing NaCl (4%)
and oxacillin (6 g/ml) or methicillin (10 g/ml) [Book ref. 120,
p. 151].
Heteroresistance refers to the expression of resistance in only
a minority of cells in a genetically resistant population; most
strains of MRSA are heteroresistant. [Mechanisms of heteroresistance: AAC (1994) 38 724728.]
Nasal MRSA in carriers may be eliminated by MUPIROCIN; hair
and skin may be disinfected by povidoneiodine (see IODINE) or
by 4% CHLORHEXIDINE. Some strains of MRSA exhibit plasmidencoded resistance to mupirocin and/or to chlorhexidine.
MRSA is a serious problem in many areas. Levels of MRSA
are low e.g. in Holland where control includes strict isolation
of infected/colonized patients [e.g. RMM (1998) 9 109116].
[Rapid discrimination between methicillin-sensitive and
methicillin-resistant S. aureus by intact cell mass spectroscopy:
JMM (2000) 49 295300.]
[Multilocus sequence typing of methicillin-resistant and
methicillin-sensitive S. aureus: JCM (2000) 38 10081015.]
[Rapid (1 hour) detection of MRSA without prior culture:
JCM (2004) 42 18751884.]
[Rapid detection of mecA-positive and mecA-negative
coagulase-negative staphylococci by an anti-PBP 2a slide latex
agglutination test: JCM (2000) 38 20512054.]
[Genotyping of European isolates of MRSA by fluorescent
amplified fragment length polymorphism analysis and PFGE:
JMM (2001) 50 588593.]
MS ring See FLAGELLUM (a).
MscL channel See MECHANOSENSITIVE CHANNEL.
msDNA See RETRON.
MseI A RESTRICTION ENDONUCLEASE; T/TAA.
MSHA Mannose-sensitive haemagglutination (see FIMBRIAE).
MspI See RESTRICTION ENDONUCLEASE (table).
MSU Mid-stream urine (see URINARY TRACT INFECTION).
MSV MAIZE STREAK VIRUS.
MSX L-Methionine-DL-sulphoximine: an inhibitor of glutamine
synthetase and hence of AMMONIA ASSIMILATION via the GS/
GOGAT pathway.
MT Microtubule (see MICROTUBULES).
mtDNA Mitochondrial DNA (see MITOCHONDRION).
MTOC MICROTUBULE-ORGANIZING CENTRE.
(mu) (1) An abbreviation for micro- (i.e. one-millionth).
(2) MICRON. (3) SPECIFIC GROWTH RATE. (4) One of the symbols
used to designate the exponential growth rate constant see
GROWTH (a). (cf. BACTERIOPHAGE MU.)
Mu See BACTERIOPHAGE MU.
mu chain (immunol.) See HEAVY CHAIN.
2 circle Syn. TWO-MICRON DNA PLASMID.
mu particle The trivial name for certain bacteria (see CAEDIBACTER and PSEUDOCAEDIBACTER) which are endosymbionts in
strains of Paramecium and which confer the MATE KILLER
characteristic.
2 plasmid See TWO-MICRON DNA PLASMID.
3 plasmid See THREE-MICRON DNA PLASMID.
mucA gene (1) See SOS SYSTEM. (2) See ALGINATE.
Mucambo virus See ALPHAVIRUS.
mucate A salt of MUCIC ACID.
mucB gene See SOS SYSTEM.
mucic acid HOOC(CHOH)4 COOH. It is obtained e.g. by the
oxidation of galactose.
muciferous body See MUCOCYST.
mucigel
mucigel A mucilaginous layer covering the root tips and root
hairs of plants; it is composed mainly of pectin-like polysaccharides and is produced by the epidermal cells of the root tips.
The mucigel may protect against desiccation, aid in the uptake of
plant nutrients, and help to bind soil particles; it often contains
large numbers of bacteria. [Book ref. 38, pp. 565568.]
mucigenic body See MUCOCYST.
mucocutaneous leishmaniasis LEISHMANIASIS in man and other
animals in which the pathogen gives rise (in man) to invasive granulomatous lesions primarily in the oral/nasal mucous
membranes; in man the disease may follow an earlier, apparently cured, episode of CUTANEOUS LEISHMANIASIS with a latent
period of up to many years. The disease occurs mainly in South
America where it is called espundia, the causal agent being
Leishmania braziliensis; a mucocutaneous leishmaniasis caused
by L. donovani occurs in parts of Africa.
Diagnosis may involve e.g. the MONTENEGRO TEST; pentavalent
ANTIMONY compounds and/or antibiotics (e.g. amphotericin B)
may be used for treatment.
mucocyst (muciferous body; mucigenic body) In many ciliates
and some flagellates: a small, sac-like organelle which, when
appropriately stimulated, discharges a mucoid material through
a pore at the cell surface. In ciliates the mucocyst is an
invagination of the outermost membrane, the closed, inner part
of the sac being located in the cytoplasm; mucocysts often occur
in longitudinal rows parallel to the rows of kinetosomes. In some
species mucocysts may be involved e.g. in cyst formation.
mucoid Viscous; slimy; mucus-like. The term is often applied to
the colonies of certain capsulated bacteria (see CAPSULE; see also
CYSTIC FIBROSIS).
mucolytic agent A chemical agent used e.g. on a sample of
sputum prior to use of the sample as an inoculum on a culture
plate; the purpose of the agent is to liquefy the sputum so
that (i) the sputum can be manipulated, and (ii) any target cells
within the sputum will be exposed to reagents.
Mucolytic agents include dithiothreitol [example of use: JCM
(1997) 35 193196] and N-acetyl-L-cysteine [examples of use:
JCM (1999) 37 175178; JCM (1999) 37 137140].
mucopeptide (glycosaminopeptide) (1) Syn. PEPTIDOGLYCAN. (2)
Any peptide-containing mucopolysaccharide.
mucopolysaccharide (glycosaminoglycan) A polysaccharide that
contains a high proportion of amino sugars and (commonly)
uronic acids: e.g. HYALURONIC ACID.
mucoprotein A protein covalently linked to amino sugars.
mucopurulent Containing mucus and pus.
Mucor A genus of fungi (order MUCORALES) which typically
occur as saprotrophs on soil, vegetable matter and dung. The
vegetative thallus is usually a branched, aseptate mycelium,
though some species are dimorphic. The organisms form
ZYGOSPORES (see also SPOROPOLLENIN); many species exhibit HETEROTHALLISM (see also COMPATIBILITY sense 2 and PHEROMONE).
(For M. miehei and M. pusillus see RHIZOMUCOR.)
Mucoraceae See MUCORALES.
Mucorales An order of fungi (class ZYGOMYCETES) which occur
as saprotrophs on decaying vegetable matter, soil or dung, or as
parasites or pathogens of plants or animals (see e.g. ZYGOMYCOSIS). The vegetative thallus is typically a well-developed aseptate
mycelium; some species (e.g. Mucor rouxii, other species of
Mucor, Mycotypha spp) are DIMORPHIC FUNGI (sense 1). The
organisms commonly form asexually derived spores in sporangia
and/or sporangiola. Most species form ZYGOSPORES (q.v.) cf.
Saksenaeaceae (below).
Nine families are recognized [Book ref. 64, pp. 247248] on
the basis of reproductive structures:
multiplex PCR
loss during an epiphytotic is less likely than it would be for
a genetically uniform susceptible cultivar. [Review: ARPpath.
(1985) 23 251273.]
multiloculate (multilocular) Consisting of or having many LOCULES: see e.g. FORAMINIFERIDA.
multilocus enzyme electrophoresis (MEE) A method in which
the electrophoretic mobilities of a range of enzymes from one
organism are compared with those of equivalent enzymes from
one or more closely related organisms; MEE is used e.g. for
TYPING microorganisms. In this method, enzymes are isolated
and tested under conditions in which enzymic activity is retained;
enzymes can be identified in gels by specific colour-generating
substrates.
Variation in the electrophoretic mobility of a given enzyme
can arise e.g. when a variant form of the enzyme is specified
by a different allele of the enzyme-encoding gene; such an
enzyme which may exhibit a different mobility when only a
single amino acid differs is called an alloenzyme.
multilocus sequence typing See MLST.
multipartite virus Syn. MULTICOMPONENT VIRUS.
multiple cloning site Syn. POLYLINKER.
multiple drug resistance See ANTIBIOTIC.
multiple fission A type of fission in which one cell gives rise
to many cells. Multiple fission may involve repeated BINARY
FISSION within a common envelope (as e.g. in CYANOBACTERIA
of section II), or it may involve a series of nuclear divisions
followed by the incorporation of each nucleus in a separate
daughter cell (see e.g. SCHIZOGONY).
multiple sclerosis A chronic demyelinating disease of the CNS
in humans. It is generally believed to be an autoimmune disease,
possibly triggered by viral infection; it has been suggested that
any of various enveloped viruses may be able to trigger the
autoimmune response which could be mounted against host
lipids incorporated (with viral proteins) in the viral envelope
[Nature (1986) 321 386]. (See also HTLV; INOUEMELNICK VIRUS;
MORBILLIVIRUS; cf. THEILERS MURINE ENCEPHALOMYELITIS VIRUS.)
multiple-tube method (most probable number (MPN) method)
A method for estimating the number of viable organisms (usually
bacteria) suspended in a liquid. The method is used e.g. for the
bacteriological examination of natural and treated waters; for this
purpose, one of several possible procedures is as follows. Five
tubes, each containing a suitable liquid growth medium, are each
inoculated with a fixed volume of the sample water (or a dilution
of it). Another five tubes, containing the same medium, are each
inoculated with a smaller fixed volume of the sample, and further
sets of tubes are similarly inoculated with progressively smaller
volumes. Following incubation, each tube is examined for the
presence or absence of growth. (It is assumed that growth will
occur in any tube which receives at least one viable organism.)
Growth usually occurs in those tubes inoculated with the larger
volumes of the sample since these tubes are more likely to
have received at least one viable organism in the inoculum. The
number of cells in the original sample can be calculated from
the pattern of positive (growth) and negative (no growth) tubes
by the use of statistical (probability) tables; if a diluted sample
were used, the count indicated by the tables is multiplied by the
dilution factor. By using a selective medium in the tubes it is
possible to estimate the numbers of a particular type of organism
in the sample. The multiple-tube method is characterized by a
large sampling error. (See also COUNTING METHODS.) [Improved
method of computing MPNs: AEM (1983) 45 16461650.]
multiplex PCR A form of PCR in which two or more different
targets are amplified, simultaneously, in a single assay. The reaction mixture usually contains two types of primer for each target;
multiplicity of infection
muramic acid 3-O-Lactylglucosamine: see PEPTIDOGLYCAN.
muramidase An enzyme which cleaves glycosidic bonds in
PEPTIDOGLYCAN: see e.g. LYSOZYME. A muramidase obtained from
the bacteriolytic hyphomycete Chalara (D Chalaropsis) sp
is commonly used in studies on peptidoglycan; this enzyme
hydrolyses the same glycosidic bond as lysozyme but differs
e.g. in substrate specificity [JBC (1967) 242 55865590].
muramyl dipeptide See MDP.
murein Syn. PEPTIDOGLYCAN.
murein lipoprotein Syn. BRAUN LIPOPROTEIN.
mureinoplast Any Gram-negative bacterial cell from which the
outer membrane, but not the peptidoglycan, has been removed.
murid (beta) herpesvirus 1 See BETAHERPESVIRINAE.
murid herpesvirus 2 See BETAHERPESVIRINAE.
muriform Refers to a spore which has both transverse and
longitudinal septa.
murine Of or pertaining to rats or mice (Muridae).
murine cytomegalovirus group See BETAHERPESVIRINAE.
murine encephalomyocarditis virus See CARDIOVIRUS.
murine hepatitis virus See CORONAVIRIDAE.
murine leukaemia viruses (MLVs; MuLVs) A group of type
C retroviruses (subfamily ONCOVIRINAE), nearly all of which
are replication-competent and v-onc (but cf. ABELSON MURINE
LEUKAEMIA VIRUS), and some of which can induce e.g. lymphatic
leukaemia in mice after a long latent period (see e.g. MOLONEY
MURINE LEUKAEMIA VIRUS). (All replication-competent murine
type C retroviruses are termed murine leukaemia viruses,
although most are usually non-leukaemogenic [Book ref. 114,
p. 70].)
MuLV-induced leukaemogenesis requires viraemia (i.e., it
requires expression and replication of the virus) and an active
cellular immune response to the MuLV env gene product; it has
been suggested that chronic immune stimulation may be a factor
in leukaemogenesis. Although the env gene product is thought
to play a direct role in leukaemogenesis, it has been shown that
the primary oncogenic determinant in one MuLV lies outside
the env region possibly in the LTR [JV (1983) 47 317328].
(See also MCF VIRUSES.)
MuLVs have given rise to a range of defective, often
acutely oncogenic variants: see e.g. FRIEND VIRUS, HARVEY MURINE
in some cases, however, one primer can be shared by two targets e.g. 16S rRNA sequences from two species, Bacteroides
forsythus and Prevotella intermedia, were simultaneously amplified with one forward primer (a BROAD-RANGE PRIMER common
to both species) and two species-specific reverse primers [JCM
(1999) 37 16211624].
Owing to the use of multiple primers, it is particularly
important to ensure the absence of complementarity between
the 30 ends of the primers in order to avoid the formation of
PRIMER-DIMERS.
The possibility of competition between different targets in a
multiplex PCR may be investigated by adding a few copies of
another target which is amplifiable but distinct from the other
targets. Failure of this target to amplify (when other(s) are
positive) would suggest that competition/inhibition has affected
the efficiency of amplification; in these circumstances, the failure
of amplification of other target(s) in the same assay would not
be considered meaningful [JCM (1998) 36 191197].
Examples of the use of multiplex PCR include: detection of chlamydiae [JCM (1999) 37 575580]; detection of
vancomycin-resistance genes in enterococci [JCM (1999) 37
20902092]; detection of mecA and coa genes in Staphylococcus aureus [JMM (1997) 46 773778]; detection of different
types of virus in cerebrospinal fluid (CSF) [JCM (1997) 35
691696]; and detection of HIV-1, HIV-2, HTLV-I and HTLV-II
[PNAS (1999) 96 63946399].
The amplification of two targets is also referred to as duplex
PCR.
multiplicity of infection (moi) The ratio of virions to susceptible
cells in a given system; e.g., a high moi means a large number
of virions per cell.
multiplicity reactivation See REACTIVATION.
multiseriate Arranged in or forming several rows; more than one
cell wide.
multisite mutation A MUTATION which involves the alteration of
two or more contiguous nucleotides. (cf. POINT MUTATION.)
multivalent vaccine Syn. POLYVALENT VACCINE.
Multivalvulida See MYXOSPOREA.
MuLV MURINE LEUKAEMIA VIRUS.
m MICROMETRE.
2m circle (2m plasmid) Syn. TWO-MICRON DNA PLASMID.
mumps (contagious, infectious or epidemic parotitis) An acute
infectious human disease which affects mainly children; it is
caused by a PARAMYXOVIRUS. Transmission occurs by droplet
infection. Incubation period: 23 weeks. The disease ranges
from subclinical to severe. Typical symptoms include fever with
pain and swelling of one or more salivary glands (usually the
parotid). Common complications include MENINGITIS, often with
mild encephalitis, and orchitis; oophoritis, mastitis, pancreatitis
etc may also occur. Infection seems to confer life-long immunity.
Lab. diagnosis: serological tests (CFT, HAI test) for mumps
virus antibodies; isolation of mumps virus e.g. from pharynx
or urine.
mundticin A 43-amino-acid class IIa BACTERIOCIN produced by
Enterococcus mundtii.
mungbean yellow mosaic virus See GEMINIVIRUSES.
mupirocin (pseudomonic acid A) An antibiotic produced by
strains of Pseudomonas fluorescens. It is active against staphylococci and streptococci associated with skin infections, and
the topically-applied antibiotic has been shown to be effective
against experimental infection of surgical wounds by Staphylococcus aureus [JAC (1985) 16 519526]. Mupirocin appears
to act by inhibiting isoleucyl-tRNA synthetase. [Review: JAC
(1987) 19 15.]
498
mutasynthesis
Murray Valley fever (Australia X disease) An acute human
disease caused by a flavivirus (see FLAVIVIRIDAE) and transmitted
by mosquitoes (e.g. Culex annulirostris); it occurs in parts of
Australasia. The disease is usually a mild, febrile condition, but
encephalitis may occur and may be fatal in young children. Birds
may act as a reservoir of infection.
Murraya See LISTERIA.
muscarine (muscarin) A quaternary ammonium derivative of
tetrahydrofuran produced e.g. by Amanita muscaria (the fly
agaric) and Inocybe spp; it is toxic to flies, and infrequently
causes a fatal intoxication in humans. (See also MYCETISM.)
muscicolous Growing on mosses.
mushroom (1) Loosely: any umbrella-shaped fungal fruiting
body; such a fruiting body consists of a horizontally orientated,
circular PILEUS supported, at its centre, by a vertical, columnar
STIPE. Mushroom is often reserved for those fruiting bodies in
which the pileus has radially arranged lamellae (see LAMELLA)
or lamella-like structures on its underside.
(2) Any AGARIC.
(3) The (edible) fruiting body of Agaricus brunnescens, the
common cultivated mushroom (see AGARICUS and MUSHROOM
CULTIVATION). (See also MUSHROOM DISEASES.)
(4) Any edible mushroom including e.g. ENOKITAKE, OYSTER
FUNGUS and SHII-TAKE. (cf. TOADSTOOL.)
mushroom cultivation The mycelium of the edible mushroom
Agaricus brunnescens (D A. bisporus) is cultivated on composted material traditionally a mixture of straw and horse
manure (see COMPOSTING; [SEM of flora: JAB (1983) 55
293304]). After an initial composting period, the compost
undergoes peak-heating (pasteurization) to ca. 5060 C; during this stage thermophilic actinomycetes and fungi continue to
grow, but the number of mesophiles including many mushroom parasites and pathogens is reduced. (See also OLIVEGREEN MOULD.) The compost is then allowed to cool to ca. 25 C
and inoculated with SPAWN of a selected strain of A. brunnescens.
After ca. 14 days, during which the mycelium of A. brunnescens
grows through the compost, a casing layer of soil or a mixture of peat and chalk or limestone is spread over the compost.
The temperature is maintained at ca. 25 C (RH >90%) for ca.
1 week. When the mycelium reaches the surface of the casing
layer, the temperature and RH are allowed to fall (e.g. to ca.
1618 C or less, RH 8090%) to induce initiation of fruiting.
Mature fruiting bodies begin to appear ca. 3 weeks after casing,
and then appear in flushes at intervals of ca. 710 days. During
the growth of A. brunnescens the previous (thermophilic) flora
declines, and progressive colonization by mesophilic fungi (e.g.
species of Aspergillus and Trichoderma) occurs [TBMS (1980)
74 465470].
The composting and pasteurization processes appear to be
necessary to provide low C:N ratios with high levels of
organic nitrogen (ammonia being inhibitory to A. brunnescens).
The microbial population established during these stages may
act as a direct source of nutrients for A. brunnescens, which
produces a variety of extracellular enzymes (including a bN-acetylmuramidase) that can lyse and degrade bacteria [JGM
(1984) 130 761769] and fungal mycelium [JGM (1985) 131
17351744]. The casing is necessary to switch growth of
A. brunnescens from vegetative to reproductive. This switch
appears to be associated with the activities of bacteria (especially
pseudomonads) in the casing layer, possibly involving the
removal by the bacteria of certain self-inhibitory fungal
metabolites; the casing may also serve to trap some volatile
product(s) of A. brunnescens or other fungi in the compost
[Book ref. 39, p. 291].
Mutatest
accuracy in the polymerizing (nucleotide selection) activity
and/or in the proof-reading activity of the enzyme.
Other mutator genes in E. coli include genes involved in the
MISMATCH REPAIR system.
Another mutator, designated mutT, specifically increases the
level of AT ! CG transversions.
[Escherichia coli mutator genes: TIM (1999) 7 2936.]
Some DNA polymerase mutants of E. coli exhibit mutation
rates which are lower than those in wild-type cells; the corresponding gene is then called an antimutator gene. An antimutator
gene product presumably permits fewer errors than occur normally during replication possibly by increasing the efficiency
of the proof-reading/editing function of the enzyme.
(See also BACTERIOPHAGE MU.)
mutator phage Any phage which, on infection of a host bacterium, causes an increase in the rate of mutation in the host
cell (see BACTERIOPHAGE MU and BACTERIOPHAGE D108).
mutD gene See DNA POLYMERASE.
mutH gene See MISMATCH REPAIR.
Mutinus See PHALLALES.
mutL gene See MISMATCH REPAIR.
mutS gene See MISMATCH REPAIR.
mutualism SYMBIOSIS (sense 1) in which both symbionts derive
benefit from the association. (cf. COMMENSALISM.) Some authors
reserve the term for an obligatory association, i.e., an association of organisms which, in nature, cannot live independently.
Optional (facultative) mutualism is sometimes called PROTOCOOPERATION.
MV-L3 phage group (L3 acholeplasmavirus group) A group of
MYCOPLASMAVIRUSES probably belonging to the PODOVIRIDAE.
Type member: bacteriophage MV-L3 (D MVL3; D L3 strain
L3). The MV-L3 virion has a polyhedral head (diam. ca. 60 nm)
with a short tail (ca. 20 9 nm) attached at one vertex via a
collar; it includes five or more proteins and ca. 2% by weight
of fucose. Genome: linear dsDNA (MWt 2.6 107 ). Host:
Acholeplasma laidlawii ; plaques clear, minute. Infected cells
are killed but not lysed; progeny virions seem to be released
in membrane vesicles which subsequently rupture.
Mx protein See INTERFERONS.
mxi-spa genes See DYSENTERY.
myalgia Muscle pain.
Myambutol Syn. ETHAMBUTOL.
myb
An ONCOGENE originally identified as the transforming
determinant in avian myeloblastosis virus (AMV: see AVIAN
ACUTE LEUKAEMIA VIRUSES); v-myb is an altered form of a cellular
sequence amv, differing from amv in gene structure, transcript
structure, gene product structure, and in the intracellular location
(nucleus) of its product [Book ref. 113, pp. 143151]. v-mybC
AMV can transform chicken haematopoietic cells in culture, but
differs from other acutely transforming retroviruses in that it
does not transform fibroblasts in culture; it causes a rapidly fatal
leukaemia only in chickens.
myc
An ONCOGENE originally identified as the transforming
determinant of avian myelocytomatosis virus (MC29: see AVIAN
ACUTE LEUKAEMIA VIRUSES). The MC29 v-myc product is a gagmyc fusion protein (P110gagmyc ) which has no protein kinase
activity; it binds to dsDNA and occurs possibly as a chromatin
component in the nucleus. In humans, c-myc is located on
chromosome 8 and is involved in the pathogenesis of BURKITTS
LYMPHOMA. In chickens, c-myc activation by AVIAN LEUKOSIS
VIRUSES appears to result in the development of lymphoid
leukosis.
mycangium Syn. MYCETANGIUM.
m 0.69
n n0
Mycobacterium
Mycelia Sterilia See AGONOMYCETALES.
mycelium A group or mass of discrete hyphae (see HYPHA):
the form of the vegetative thallus in many types of fungi
and in certain bacteria (see ACTINOMYCETALES). (See also
AERIAL MYCELIUM, SPROUT MYCELIUM; SUBSTRATE MYCELIUM; cf.
PLECTENCHYMA.)
Mycena See AGARICALES (Tricholomataceae) and BIOLUMINESCENCE.
mycetangium (mycangium) In certain insects: a specialized
region within which symbiotic fungi are carried; see e.g.
AMBROSIA FUNGI and WOODWASP FUNGI.
mycetism (mycetismus) Poisoning due to the ingestion of certain
mushrooms (MUSHROOM sense 1) e.g. the poisonous species of
Amanita or Cortinarius. (cf. MYCOSIS, MYCOTOXICOSIS; see also
e.g. AMATOXINS, MUSCARINE and PHALLOTOXINS.) Mycetism can
occur in e.g. sheep and cattle as well as in humans; thus, e.g.
the toxins in Cortinarius speciosissimus are known to cause
renal failure in both humans and sheep. (See also ORELLANIN
POISONING.)
mycetismus Syn. MYCETISM.
mycetocyte In certain invertebrates, particularly insects: a specialized cell which contains intracellular bacterial or fungal
symbionts; if the endosymbiont is a bacterium the term BACTERIOCYTE may be used although mycetocyte is often used
regardless of the nature of the endosymbiont. Mycetocytes may
be irregularly distributed in certain tissues (e.g. the gut lining) or
they may be aggregated into specialized organelles (mycetomes)
which are usually associated with the gut. In at least some cases
the microflora of the mycetome supplies essential nutrients to the
insect host. (See also MYCETANGIUM and TROPHOSOME.) [Molecular biology of symbiotic bacteria in aphid mycetocytes: MS
(1986) 3 117120.]
mycetoma (1) Syn. MADUROMYCOSIS. (2) (fungus ball) A tumourlike mycelial mass formed in the tissues in certain mycoses (see
e.g. ASPERGILLOSIS and COCCIDIOIDOMYCOSIS).
mycetome See MYCETOCYTE.
mycetophagous Syn. MYCOPHAGOUS.
Mycetozoa A subphylum (phylum GYMNOMYXA) comprising two
classes: Eumycetozoa (see EUMYCETOZOEA) and Acrasea (see
ACRASIOMYCETES).
Mycoacia See APHYLLOPHORALES (Corticiaceae).
mycobacteriophage Any BACTERIOPHAGE which can infect one
or more Mycobacterium spp. Most mycobacteriophages have
a hexagonal head and a non-contractile tail (contractile in
I3), and many are readily inactivated by organic solvents.
Mycobacteriophages include both temperate and virulent types;
in certain cases phage progeny may be released from the living
host cell. [Book ref. 54, pp. 326342.]
Mycobacterium A genus of Gram-positive, aerobic to microaerophilic, non-motile, asporogenous bacteria (order ACTINOMYCETALES, wall type IV) that are acid-fast during at least some
stage of growth.
Cells: typically straight or curved rods, ca. 0.20.8
110 m, but may occur as coccoid forms, branched rods or
fragile filaments; some strains are capsulated (see also MYCOSIDE
C). Individual cells may stain uniformly or may exhibit banding or beading. The CELL WALL contains MYCOLIC ACIDS (see also
CORD FACTOR, WAX D and PEPTIDOGLYCAN).
Some strains form CAROTENOID pigments: see PHOTOCHROMOGEN and SCOTOCHROMOGEN.
Species of Mycobacterium occur in soil as free-living saprotrophs, in water [review: JAB (1984) 57 193211], on plants,
and as parasites and pathogens of man and other animals (including fish) (see e.g. BURULI ULCER, JOHNES DISEASE, LEPROSY, SCROFULA and TUBERCULOSIS).
Metabolism is respiratory and, typically, chemoorganotrophic although chemolithotrophic strains of e.g. M. marinum and M. smegmatis have been reported. Nutritionally,
mycobacteria are generally not fastidious; sources of carbon
and nitrogen include e.g. sugars, hydrocarbons and amino acids.
In a number of species glycerol and asparagine are preferred
sources of C and N, respectively. Growth may be stimulated
Mycobacterium
M. branderi. SG; non-pigmented/scotochromogenic. Typical
tests: arylsulphatase Cve; niacin ve; reduction of nitrate
weak; Tween hydrolysis ve; growth 2545 C Cve. [Original
description of species: IJSB (1995) 45 549553.] M. branderi
has been isolated from the respiratory tract on a number of
occasions and may be a causal agent of disease.
M. celatum. SG; non-pigmented. Typical tests: catalase (68 C)
Cve; arylsulphatase variable; niacin ve; reduction of nitrate
ve; Tween hydrolysis ve; T2H test Cve. [Original description
of species: IJSB (1993) 43 539548.]
Strains of M. celatum have been classified into three types
(IIII) on the basis of RFLP analysis. Type I strains may give
false-positive results with a commercial probe for M. tuberculosis [JCM (1994) 32 536538].
M. celatum has been isolated from a range of infections, some
in patients with AIDS [e.g. Lancet (1994) 344 332; Lancet (1994)
344 10201021].
M. chelonei (D M. chelonae). RG; non-pigmented. Similar to
M. fortuitum but e.g. does not grow at 42 C (optimum growth
temperature 25 C) and does not reduce nitrate. M. chelonei
has been isolated e.g. from infected wounds.
M. farcinogenes. RG. Resembles M. fortuitum (on the basis
of DNA homology studies). A causal agent of bovine FARCY.
M. flavum. See XANTHOBACTER.
M. fortuitum. RG; non-pigmented. Typical tests: arylsulphatase Cve; growth at 42 C Cve; Tween hydrolysis variable;
reduction of nitrate Cve. An opportunist pathogen. [DNA relatedness study of the M. fortuitumM. chelonae complex: IJSB
(1986) 36 458460.]
M. gordonae (previously called M. aquae). SG; scotochromogen. The organism occurs in water, and is an occasional cause
of pulmonary disease; it is not susceptible to isoniazid or pyrazinamide but is sensitive to some other antimycobacterial drugs. A
DNA probe (for identifying isolates) is available commercially.
M. haemophilum. SG; non-pigmented. Requires haemin for
growth. Growth occurs at 30 C, not at 37 C. Causes disease
in the immunosuppressed and in healthy children. [Clinical and
laboratory aspects of M. haemophilum infections: RMM (1998)
9 4954.]
M. interjectum. SG; scotochromogen. Typical tests: catalase (68 C) Cve; arylsulphatase variable; niacin ve; reduction of nitrate ve; Tween hydrolysis variable; growth at
3137 C Cve; T2H test Cve. [Original description of species:
JCM (1993) 31 30833089.]
M. interjectum was first isolated from a child with chronic
submandibular lymphadenitis (and a positive TUBERCULIN TEST).
Partial resection of the lymph node and treatment with antituberculosis drugs failed to resolve the infection; subsequent
total resection of the node and treatment with isoniazid, clarithromycin and protionamide was successful. M. interjectum has
been associated with cervical lymphadenitis in a child [JCM
(2001) 39 725727].
M. intracellulare. SG; non-pigmented. Similar to M. avium
but typically arylsulphatase Cve, catalase (68 C) Cve. Tween
hydrolysis ve. Growth occurs at 2540 C (some strains grow
at 4045 C). (See also MAC.)
M. kansasii. SG; usually photochromogenic. Typical tests:
arylsulphatase Cve; catalase (68 C) Cve; growth at 2540 C
Cve (some strains grow at 42 C); niacin ve; reduction of
nitrate Cve; T2H test Cve; Tween hydrolysis Cve.
M. kansasii can cause human disease similar to pulmonary
tuberculosis; moreover, M. kansasii can cross-react with
M. tuberculosis in the AMTDT [JCM (1999) 37 175178].
Mycoplasma
ve; growth at 52 C Cve; Tween hydrolysis Cve; T2H test Cve.
Found e.g. in soil. Reported to be pathogenic in lung (several
cases); skin and lymph nodes; and breast tissue [JCM (1992) 30
10361038].
M. triplex. SG; non-pigmented. Isolated from various clinical
specimens. [Description of species: JCM (1996) 34 29632967.]
[M. triplex associated with infection in a liver transplant patient:
JCM (2001) 39 20332034.]
M. tuberculosis. SG; aerobic. Non-pigmented. Typical test
results: catalase (68 C) ve; growth at 42 C ve; growth at
37 C Cve; growth enhanced by glycerol and by pyruvate; niacin
Cve; reduction of nitrate Cve; Tween hydrolysis variable; sensitive to pyrazinamide. Usually forms rough, raised, whitish/pale
buff colonies (eugonic growth).
A casual agent of TUBERCULOSIS.
[Genome sequence of M. tuberculosis, strain H37rv: Nature
(1998) 393 537544.] The insertion sequence IS6110 (q.v.) is
frequently used for TYPING isolates of M. tuberculosis.
M. ulcerans. SG; pigmentation variable. Typical test results:
catalase (68 C) Cve; growth at 30 C Cve; growth at 37 C ve;
niacin variable; reduction of nitrate ve; Tween hydrolysis ve.
This species is found in tropical regions e.g. on vegetation; it
causes BURULI ULCER.
M. xenopi. SG; pigmentation variable. Found in water, and
able to cause lesions in the (human) lung. Does not grow at 25 C,
grows poorly at 37 C, and has an optimum growth temperature
of ca. 4245 C.
mycobactins A family of complex, lipophilic compounds which
occur in the cell envelope in most species of Mycobacterium
(not in M. paratuberculosis or in some strains of M. avium);
they chelate trivalent metal ions, particularly solubilized ferric
ions, and are believed to function in iron transport iron being
released after enzymic reduction to the ferrous form. For in vitro
growth M. paratuberculosis needs mycobactin or e.g. ferric
ammonium citrate. [Structure of mycobactins: Book ref. 54, pp.
242245.] (See also EXOCHELINS and SIDEROPHORES.)
Related compounds occur in Nocardia.
mycobiont A fungal symbiont e.g. in a LICHEN or MYCORRHIZA.
Mycobionta Syn. EUMYCOTA.
Mycocalia See NIDULARIALES.
Mycocaliciaceae See CALICIALES.
mycocecidia GALLS induced by fungi.
Mycocentrospora See HYPHOMYCETES; see also CROWN ROT.
mycochrome See PHOTOINDUCTION and PHOTOINHIBITION.
mycodextran Syn. NIGERAN.
Mycogone See HYPHOMYCETES; see also BUBBLE DISEASES.
mycoherbicide See BIOLOGICAL CONTROL.
mycolic acids a-Substituted, b-hydroxylated fatty acids (having
the general formula R0 CHOH.CHR00 .COOH), esters of which
are found in the cell walls of e.g. species of Corynebacterium,
Mycobacterium, Nocardia, and Rhodococcus; in Mycobacterium spp the mycolic acids fall within the approximate
range C60 C90 , in Nocardia C40 C60 , and in Corynebacterium
C20 C40 .
In mycobacterial mycolic acids R0 is usually a C50 C60
chain which often includes double bonds, cyclopropane rings
etc, while R00 is a C22 C24 chain. [Structure and biosynthesis:
Book ref. 54, pp. 113128. Mycolic acid patterns in various
strains of Mycobacterium: JGM (1983) 129 889891; (1984)
130 363367, 27332736.] (See also WAX D.)
[Mycolic acids in Corynebacterium spp: JGM (1984) 130
513519.]
mycology The study of FUNGI.
mycoparasite A fungus which is parasitic on other fungi. Mycoparasites include e.g. Christiansenia pallida [life history: Mycol.
(1984) 76 922]; PIPTOCEPHALIS; and Rozella spp: endobiotic and
holocarpic organisms which parasitize e.g. Polyphagus euglenae
(itself a parasite of Euglena spp) [Mycol. (1984) 76 10391048]
and other fungi and algae. Certain mycoparasites can apparently
exert some control on pathogens of higher plants e.g., in cases
of CLOVER ROT, Trichoderma viride (or e.g. Mitrula sclerotiorum)
can bring about a reduction of the numbers of sclerotia in the soil
[Bot. Rev. (1984) 50 491504]. [Susceptibility of e.g. Pythium
spp to the mycoparasite Pythium oligandrum: SBB (1986) 18
9196.] (See also CONTACT BIOTROPHIC MYCOPARASITE.)
mycophagous (mycetophagous) Fungus-eating.
mycophenolic acid An ANTIBIOTIC produced e.g. by Penicillium
brevicompactum in aerial hyphae formed on solid media [AEM
(1981) 41 729736]. It has antimicrobial and antitumour activity, blocking GMP synthesis by inhibiting the formation of
XMP from IMP (see Appendix V(a)).
Mycoplana
A genus of Gram-negative, aerobic bacteria of
uncertain taxonomic affinity; species occur e.g. in soil. The
organisms form branching filaments which fragment into irregular, flagellated rods. Some strains can fix nitrogen under
microaerobic conditions [JGM (1982) 128 20732080]. GC%:
ca. 6469. [Book ref. 46, pp. 21182119.]
mycoplasma (1) A member of the class MOLLICUTES. (cf. MOLLICUTE.) (2) A member of the genus MYCOPLASMA.
Mycoplasma A genus of cell wall-less, sterol-requiring, catalasenegative bacteria (family MYCOPLASMATACEAE) which occur as
parasites and pathogens e.g. in the respiratory and urogenital
tracts in man and other animals; diseases caused by, or associated
with, Mycoplasma spp include e.g. AIR SACCULITIS, BRONCHITIS,
CONTAGIOUS BOVINE PLEUROPNEUMONIA, GLASSERS DISEASE, NONGONOCOCCAL URETHRITIS, ovine MASTITIS, and PRIMARY ATYPICAL
PNEUMONIA (sense 2). (Mycoplasma spp are also common contaminants in TISSUE CULTURES.) Cells: typically non-motile (but
see below) and pleomorphic, ranging from spherical, ovoid or
pear-shaped (ca. 0.30.8 m diam.) to branched filamentous
forms of near-uniform diameter, several m to ca. 150 m in
length; filaments, the typical forms in young cultures under optimum conditions, subsequently transform into chains of coccoid
cells which later break up into individual cells that are capable of passing through membrane filters of pore size 0.22 m
or 0.45 m. The cells of some species have a tip structure
(possibly part of a microfibrillar cytoskeleton) which has been
thought to be involved in attachment to host cells, and which (in
motile species) appears to have a role in GLIDING MOTILITY the
tip always pointing in the direction of motion.
The attachment organelle and cytoadherence proteins of M.
pneumoniae have been detected by immunofluorescence microscopy [JB (2001) 183 16211630].
The trilaminar cytoplasmic membrane contains sterols (in
addition to e.g. phospholipids and proteins) thus rendering the
cells susceptible to POLYENE ANTIBIOTICS and to lysis by e.g.
digitonin (which complexes sterols). Some species bear a capsule
or slime layer that in M. mycoides subsp mycoides being a
galactan.
Replication of the genome may precede cytoplasmic division;
hence, multinucleate filaments may exist for a time before
individual cells are delimited by constriction. Budding can also
occur.
Most Mycoplasma spp are facultatively anaerobic, some
apparently being obligately anaerobic on primary isolation. All
species are chemoorganotrophic. Fermentative species can use
503
mycovirus
HISTOPLASMOSIS; LOBOMYCOSIS; MADUROMYCOSIS; ONYCHOMYCOSIS; PARACOCCIDIOIDOMYCOSIS; PHAEOHYPHOMYCOSIS; PITYRIASIS
NIGRA; PITYRIASIS VERSICOLOR; RHINOSPORIDIOSIS; RINGWORM;
SPOROTRICHOSIS; WHITE PIEDRA; ZYGOMYCOSIS.
mycosis fungoides A chronic human cutaneous T-cell lymphoma. HTLV-I provirus has been detected in a very small
proportion of cases, but HTLV-I is not thought to be an aetiological agent. (cf. ADULT T-CELL LEUKAEMIA.)
Mycosphaerella A genus of fungi (order DOTHIDEALES) which
include saprotrophs and plant parasites (see e.g. BANANA LEAF
SPOT). (See also CLADOSPORIUM.)
mycotete See TERMITEMICROBE ASSOCIATIONS.
mycotic dermatitis Syn. LUMPY WOOL.
mycotoxicosis Any disease of man or animals resulting from
the ingestion of MYCOTOXINS (cf. MYCETISM; MYCOSIS). See e.g.
ALIMENTARY TOXIC ALEUKIA; DENDRODOCHIOTOXICOSIS; ERGOTISM;
LUPINOSIS, PASPALUM STAGGERS; STACHYBOTRYOTOXICOSIS; YELLOW RICE.
mycotoxin A TOXIN produced by a fungus. The term is usually
reserved for fungal metabolites that are toxic to man and/or
animals and are produced by moulds growing on foodstuffs
(cf. MYCETISM). See e.g. AFLATOXINS; ASTELTOXIN; AUROVERTINS;
CHLOROPEPTIDE; CITREOVIRIDIN; CITRININ; CYCLOPIAZONIC ACID;
ERGOCHROMES; ERGOT ALKALOIDS; OCHRATOXINS; PATULIN; PENITREMS; RUBRATOXINS; SLAFRAMINE; SPORIDESMINS; STERIGMATOCYSTIN; TRICHOTHECENES; XANTHOMEGNIN; ZEARALENONE. (cf.
IPOMEAMARONE and 4-IPOMEANOL.)
mycotrophein See CONTACT BIOTROPHIC MYCOPARASITE.
mycotrophic (1) (of plants) Refers to the plant partner in a
MYCORRHIZA. (2) (of animals) Refers to an animal (e.g. an
invertebrate) that feeds on fungi.
Mycotypha See MUCORALES.
mycovirus Any VIRUS which can infect one or more fungi.
Mycoviruses have been observed in a wide range of fungi; the
majority are isometric (diam. ca. 2550 nm) dsRNA viruses
either with monopartite genomes or with segmented genomes,
each segment being encapsidated in a separate particle. Many
of the dsRNA virions have been shown to contain an RNADEPENDENT RNA POLYMERASE. Six groups of isometric dsRNA
mycoviruses have been defined [Intervirol. (1984) 22 1723].
Group A: genome monopartite (4.86.1 kbp), virion diam. ca.
3543 nm; members: Saccharomyces cerevisiae viruses ScV-L1
(D ScV-LA) and ScV-L2; probable members: Ustilago maydis
viruses UmV-P1-H1, UmV-P4-H1 and UmV-P6-H1. Group B :
genome monopartite (8.3 kbp), virion diam. ca. 48 nm; member:
Drechslera (formerly Helminthosporium) maydis virus (HmV).
Group C : genome bipartite (1.6 and 1.4 kbp), virion diam. ca.
3035 nm; member: Penicillium stoloniferum virus S (PsV-S);
probable member: Diplocarpon rosae virus (DrV). Group D
(Gaeumannomyces graminis virus group 1): genome bipartite
(1.81.9 and 1.71.8 kbp), virion diam. ca. 35 nm; members:
G. graminis viruses GgV-019/6-A, GgV-OgA-B and GgVF6-C. Group E (Gaeumannomyces graminis virus group 2):
genome bipartite (2.22.3 and 2.02.1 kbp), virion diam. ca.
35 nm; members: G. graminis viruses GgV-F6-B, GgV-T1-A
and GgV-OgA-A. Group F : genome tripartite (ca. 3.2, 3.0 and
2.9 kbp), virion diam. ca. 3540 nm; members: Penicillium
chrysogenum virus (PcV), P. brevicompactum virus (PbV) and
P. cyaneofulvum (D P. chrysogenum) virus (Pc-fV). (Pc-fV
actually has four dsRNA segments, the 4th probably being a
variant, satellite or defective dsRNA.) Two families, Totiviridae
and Partitiviridae, have been created to accommodate isometric
dsRNA viruses with, respectively, monopartite and bipartite
genomes [Intervirol. (1986) 25 141143].
505
mycovore
Most dsRNA mycoviruses appear to have a single-layered
capsid composed of a single polypeptide species. However, a
dsRNA virus from Lentinula edodes appears to have a doubleshelled capsid [Virol. (1982) 123 93101] and to resemble
a PHYTOREOVIRUS. Other mycoviruses include e.g. Boletus
virus (a possible member of the POTEXVIRUSES) and mushroom
virus 3 (virions bacilliform, ca. 50 19 nm); DNA-containing
lytic viruses have been observed in certain lower fungi (e.g.
Rhizidiomyces [Virol. (1983) 130 1020, 2128]).
Mycoviruses are apparently transmissible only by intracellular
routes (e.g. during mating, via spores, or by hyphal anastomosis).
In many cases the host fungus shows little evidence of infection
(cf. MUSHROOM DISEASES); in certain cases virus infection may
affect the virulence of a pathogenic fungus: e.g. an isometric
dsRNA virus appears to be associated with virulence in strains of
Rhizoctonia solani [JGV (1985) 66 12211232] cf. CHESTNUT
BLIGHT and DUTCH ELM DISEASE. (See also KILLER FACTOR.)
mycovore A fungus-eating animal.
myelitis Inflammation of the spinal cord.
myeloblastosis-associated viruses See AVIAN LEUKOSIS VIRUSES.
myeloma A tumour consisting of a single clone of B LYMPHOCYTES; myelomas can occur spontaneously or they can be
induced. A given myeloma secretes Ig (paraprotein) molecules,
all of which are structurally and electrophoretically homogeneous (monoclonal); some myeloma Igs react with environmental antigens. Myeloma cells are used e.g. for HYBRIDOMA
formation. (See also BALB/C MICE.)
myeloperoxidase (MPO) A haemoprotein (MWt ca. 150000)
found e.g. in MACROPHAGES and in the azurophilic granules of
NEUTROPHILS; MPO catalyses the oxidation of halide ions to
hypohalite. [Role of MPO in oxygen-dependent microbicidal
activity of human neutrophils: Blood (1983) 61 483492.]
myo-inositol See INOSITOL.
myonecrosis (clostridial) See GAS GANGRENE.
myoneme (ciliate protozool.) A bundle, ribbon or sheet of intracellular protein microfibrils, numbers of which occur in certain ciliates; myonemes are apparently contractile and may thus
account for the observed contractility in those organisms which
contain them. Myonemes occur below the infraciliature in e.g.
Stentor and Spirostomum; in Stentor they are also known as
M bands or M fibres. (See also SPASMONEME.) Myoneme contraction appears to be related to environmental and/or intracellular
levels of calcium ions.
myosin A rod-shaped protein which occurs in most types of
eukaryotic cell; the molecule consists of six polypeptides: two
heavy chains and four light chains, the light chains occurring
at one end of the molecule and contributing to its bulbous head.
Myosin molecules can aggregate into bundles, each bundle
consisting of a number of longitudinally adjacent molecules
arranged so that head regions occur at each end. When contact
occurs between a myosin head and an ACTIN microfilament,
the head apparently undergoes a conformational change which
causes the myosin molecule (or bundle) to move relative to
the microfilament; moreover, when interposed between suitably
aligned microfilaments, a myosin bundle can apparently cause
one microfilament to move relative to the other. Continuing
movement of a microfilament relative to a myosin head seems
to involve a continual sequence of reversible changes in the
conformation of the myosin head the head repeatedly making
and breaking contact with the microfilament, and repeatedly
binding and hydrolysing ATP.
Myoviridae A family of BACTERIOPHAGES which are characterized by the possession of a long, complex, contractile tail consisting of a central tube surrounded by a coaxial contractile sheath;
Myxomycetes
PLASMODIUM which typically exhibits shuttle streaming (rhythmic
reversible flow) of its protoplasm. Multispored, usually macroscopic fruiting bodies develop from the plasmodium. Sexual
reproduction occurs in most (if not all) species, and the life
cycle typically exhibits alternate haploid and diploid phases. Myxomycetes occur in various habitats, e.g., soil, humus, rotting wood,
treebark, dung, decaying vegetation, etc. [Ecologically significant
features of myxomycetes: TBMS (1984) 83 119.]
Life cycle. A haploid spore germinates to release one or more
uninucleate myxamoebae or flagellated amoeboid cells (which
are typically biflagellated and heterokont); the two types of cell
are interconvertible e.g. myxamoebae may become flagellated
in the presence of water. The cells feed phagocytically and
osmotrophically, and divide mitotically (flagellated cells first
withdrawing their flagella); under unfavourable conditions they
may form MICROCYSTS. The amoeboid/flagellated cells function
as gametes: cells of compatible mating type fuse, and the zygote
develops into the main vegetative stage of the organism, the
plasmodium. Three main types of plasmodium are distinguished.
A protoplasmodium is microscopic, resembling a multinucleate
amoeba, and lacks reticulations or veins. Protoplasmodia occur
e.g. in ECHINOSTELIUM and many Licea spp; each gives rise
to a single fruiting body. An aphanoplasmodium (formed e.g.
by Stemonitis spp) is thin, delicate, and inconspicuous, with a
reticulum of veins leading into a broad, fan-shaped, advancing
front; aphanoplasmodia lack a slime sheath, and their protoplasm
is relatively non-granular. A phaneroplasmodium (formed e.g.
in PHYSARUM) resembles an aphanoplasmodium but is much
thicker and more robust, and is often conspicuous; its protoplasm
is very granular, and it is surrounded by a gelatinous slime
sheath traces of which are left behind on the substratum
over which the plasmodium migrates. Shuttle streaming (a
rapid, rhythmic, back-and-forth flow) of the protoplasm occurs
in aphanoplasmodia and phaneroplasmodia; in protoplasmodia
streaming is very slow and irregular. Plasmodia are commonly
yellow or white, but they may be e.g. orange, brown, red, violet
or black; the larger plasmodia may measure several centimetres
to a metre or more across. As it migrates over a substratum, the
plasmodium feeds by ingesting bacteria, microalgae, protozoa,
yeasts, particles of organic detritus etc, as well as myxamoebae
and flagellated cells of its own species (cannibalism); as it
grows, its nuclei divide synchronously. Coalescence of two or
more plasmodia may occur.
Eventually, the plasmodium gives rise to fruiting bodies (or, in
some species, to a SCLEROTIUM). Prior to fruiting, the plasmodium
generally flows out onto an exposed surface; in some species
light is apparently necessary to initiate fruiting. Three major
types of fruiting body are formed, in each of which the spores
develop in masses within a persistent or evanescent peridium. A
sporangium is a relatively small, sessile or stalked structure which
is more or less uniform in size and shape for a given species;
many sporangia usually develop from a single plasmodium. (See
e.g. ARCYRIA and STEMONITIS.) An aethalium is typically sessile,
relatively large, hemispherical or pulvinate, derived from an entire
plasmodium or from a major part of one; aethalia may vary in
size and shape even within a single species. (See e.g. LYCOGALA.)
(Pseudoaethalia, consisting of numerous compacted sporangia,
occur in some species.) A plasmodiocarp is sessile, irregularly
shaped and often branched or reticulate; it is derived from the
major veins of an aphanoplasmodium or phaneroplasmodium.
(See e.g. HEMITRICHIA.) Depending on species, fruiting bodies
may contain e.g. a CAPILLITIUM, COLUMELLA, PSEUDOCAPILLITIUM
and/or PSEUDOCOLUMELLA. In some species certain parts of the
Myxomycota
particular tissue (in histozoic species: e.g. species of Henneguya,
Kudoa, Myxobolus, Myxosoma) or body fluid (in coelozoic
species: e.g. Chloromyxum spp, Leptotheca spp, Myxidium
spp, Zschokkella floridanae). The sporoplasm grows and its
nucleus divides many times, resulting in the formation of a
multinucleate plasmodium the main vegetative stage of the
organism. Eventually, many of the nuclei in the plasmodium
each become segregated into cells (sporonts) destined to become
spores; depending on species, a sporont may develop into
a single spore (monosporous sporont) or into two or more
spores within a common envelope (the whole being termed a
pansporoblast). A sequence of nuclear divisions then ensues,
each division apparently giving rise to a somatic nucleus
and a generative nucleus. Cells containing somatic nuclei are
involved in the formation of the spore wall, polar filament(s)
and polar capsule(s), while generative nuclei are incorporated
in the sporoplasm(s) (commonly two nuclei per sporoplasm).
The mature spores may be released into the bloodstream or may
remain in situ until the host is eaten e.g. by another fish or by
a bird; in the latter case, the spores may be passed unharmed
with the birds faeces, thus possibly being transported to fresh
aquatic habitats. (cf. WHIRLING DISEASE.)
myxosporidean (Pertaining to) a protozoon of the MYXOZOA (formerly of the class Myxosporidea, subphylum Cnidospora).
Myxotheca See FORAMINIFERIDA.
Myxotrichum See GYMNOASCALES.
myxoviruses A (non-taxonomic) group of viruses: the ORTHOMYXOVIRIDAE and PARAMYXOVIRIDAE.
myxoxanthophyll See CAROTENOIDS.
Myxozoa A phylum of PROTOZOA [JP (1980) 27 3758] which
are mainly intracellular parasites of invertebrates and poikilothermic vertebrates. The organisms form spores of multicellular
origin; a spore contains one or more extrusile polar filaments,
each coiled within a separate sac (the polar capsule), and one or
more sporoplasms (amoeboid cells which are the infective forms
of the organism). The spore wall consists of one, two or three
(rarely more) valves. Two classes are recognized: ACTINOSPOREA
and MYXOSPOREA; however, since two apparently distinct organisms one from each class have been found to be different
stages in the life cycle of the same organism (see WHIRLING DISEASE), a reappraisal of myxozoan taxonomy may be necessary
[discussion: JP (1985) 32 589591]. (See also MICROSPORA and
ASCETOSPORA.)
MZ B cells MARGINAL ZONE B CELLS (q.v.).
508
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
N
N Asparagine (see AMINO ACIDS).
N-end rule The observed relationship between the N-terminal
amino acid of a protein and the half-life of that protein in vivo. In
Escherichia coli, for example, proteins whose N-terminal amino
acid is either arginine or lysine are characterized by a short halflife; early degradation of such proteins may be avoided in strains
mutant in the AAT GENE.
n. gen. See GENUS NOVUM.
N-Serve See NITRAPYRIN.
n. sp. See SPECIES NOVA.
N-type starter See LACTIC ACID STARTERS.
NA Numerical aperture: see RESOLVING POWER.
Na+ -ATPase See ION TRANSPORT and SODIUM MOTIVE FORCE.
Na+ -motive force See SODIUM MOTIVE FORCE.
Na+ pump See ION TRANSPORT.
nabam (dithane D-14) Disodium ethyleneBISDITHIOCARBAMATE,
an agricultural antifungal agent sometimes used in conjunction
with zinc sulphate and lime when ZINEB is formed.
nactins See MACROTETRALIDES.
NAD (coenzyme I; cozymase) Nicotinamide adenine dinucleotide (formerly known as diphosphopyridine nucleotide, DPN).
NAD is an important coenzyme, functioning as a hydrogen
carrier in a wide range of redox reactions; the H is carried on
the nicotinamide residue (see figure). The oxidized form of the
coenzyme is written NAD+ , the reduced form as NADH (or
NADH + H+ ); hence:
the HEXOSE MONOPHOSPHATE PATHWAY, by the isocitrate dehydrogenase reaction of the TCA CYCLE, and by PHOTOSYNTHESIS
in photosynthetic eukaryotes. (See also TRANSHYDROGENASE.)
[NADPH production and consumption in yeasts: JGM (1983)
129 953964.]
In addition to its role as a hydrogen carrier, NAD+ also functions as an ADP-ribosyl donor in ADP-RIBOSYLATION reactions.
Biosynthesis of NAD and NADP. NAD may be synthesized de
novo from aspartate and dihydroxyacetone phosphate or from
tryptophan (see NICOTINIC ACID; cf. V FACTOR). Nicotinamide
released during the degradation of NAD+ (by NAD+ nucleosidase) may be re-cycled (i.e., incorporated into new NAD
molecules) via the pyridine nucleotide salvage cycle; such a
cycle may also be operative in certain organisms which cannot
synthesize nicotinic acid/nicotinamide de novo (e.g. Bordetella
pertussis [AvL (1984) 50 3337]). NADP is synthesized by the
ATP-dependent phosphorylation of NAD by NAD+ kinase.
NAD+ kinase See NAD.
NADHUQ oxidoreductase Complex I of the mitochondrial
ELECTRON TRANSPORT CHAIN.
NADP See NAD.
Nadsonia
A genus of yeasts (family SACCHAROMYCETACEAE)
in which the cells are usually lemon-shaped; vegetative reproduction occurs by bipolar bud-fission. Pseudomycelium is not
formed. Ascus formation follows conjugation between a bud
and its mother cell; ascospores contain a prominent lipid globule and are spherical, brownish, warty or spiny, 1 or 2 per ascus.
Glucose is fermented by N. elongata and N. fulvescens, but not
by N. commutata. Nitrate is not assimilated. Maximum growth
temperature: ca. 2426 C. Species have been isolated from soil
and from the slime flux of trees. [Book ref. 100, pp. 279284.]
Naegleria
A genus of amoeboflagellates (order SCHIZOPYRENIDA). Some species (e.g. N. gruberi ) are entirely free-living. N.
fowleri (= N. aerobia, N. invades) is an opportunist pathogen
(see MENINGOENCEPHALITIS); it is ca. 10 m in diameter when
rounded, and its single nucleus contains a large central nucleolus.
(See also AMOEBOSTOME.) In N. fowleri interconversion can
occur between the amoebic form and a transient, non-dividing
biflagellate form [JB (1981) 147 217226]. Amoebae can
encyst. [ARM (1982) 36 101123.]
NH2
N
N
N
CONH2
O
O
1
H
H
2
OH
5
CH2
H
+
N
CONH2
+2H
2H
+H
N
O
O
P
O
3
OH
adenosine mononucleotide
CH2
H
R
H
OH
OH
nicotinamide mononucleotide
NAD+
NADH
509
nafcillin
nafcillin See PENICILLINS.
naftifine See ALLYLAMINES.
NAG vibrios Non-agglutinable vibrios see NON-CHOLERA VIBRIOS.
nagana Any of a range of trypanosomiases which affect domestic
animals (e.g. cattle) in various parts of Africa and in which
the vector is a biting fly, often a species of Glossina; the
pathogens include Trypanosoma brucei, T. congolense, T. suis
and T. vivax. Symptoms typically include anaemia, cachexia,
and damage to e.g. heart, kidneys and liver; affected cattle
typically exhibit a generalized immunosuppression. Abortion
and infertility are common in certain areas.
Naglers reaction A test used to detect strains of Clostridium
perfringens which produce a diffusible LECITHINASE (the atoxin). (An antigenically similar phospholipase C, which also
cleaves lecithin, is produced by C. bifermentans.) When grown
on EGG-YOLK AGAR such strains give rise to colonies each of
which is surrounded by a zone of opacity. In the Nagler reaction,
one half of a plate of egg-yolk agar is spread with anti-atoxin, and the plate is inoculated with the unknown strain the
inoculum forming a line which extends into both halves of
the plate; following incubation, strains which produce a-toxin
produce zones of opacity only in that half of the plate which does
not contain antitoxin although growth occurs in both halves of
the plate.
Nairobi sheep disease A disease of sheep and goats caused by a
virus of the genus NAIROVIRUS. It occurs mainly in East Africa.
Symptoms include haemorrhagic gastroenteritis, splenomegaly,
nephritis, and myocardial degeneration; mortality rates are high.
The virus is transmitted by the tick Rhipicephalus appendiculatus.
Nairovirus A genus of viruses of the BUNYAVIRIDAE. Host range:
various vertebrates; vectors: primarily ticks. MWts of L, M and
S RNAs: ca. 4.14.9, 1.51.9, and 0.60.7 106 , respectively.
MWts of proteins L, G1, G2 and N: ca. 145200, 7284, 3040
and 4854 103 , respectively. The genus comprises ca. 6
serogroups, including e.g. the CrimeanCongo haemorrhagic
fever group, NAIROBI SHEEP DISEASE group, and the Qalyub group.
naive (immunol.) Unprimed (cf. PRIMED).
naked (1) (of viruses) Not enveloped. (2) (of nucleic acids,
VIROIDS etc) Not associated with protein.
nalA gene See GYRASE.
nalidixic acid A QUINOLONE ANTIBIOTIC. Nalidixic acid inhibits
bacterial DNA replication (and, to a lesser extent, RNA and
protein synthesis) and causes degradation of DNA in the cell.
It acts as a specific inhibitor of GYRASE, interfering with the
function of the A subunits (cf. NOVOBIOCIN) and preventing the
breakage-and-reunion activity and hence the supercoiling and
relaxing activities of the enzyme. The drug apparently causes
the formation of a very stable gyraseDNA complex. In vitro,
treatment of the complex with e.g. SDS triggers the cleavage
of DNA strands with consequent covalent binding of the 5
ends to the A subunits; in vivo, the complex may block the
movement of replication forks [ARB (1981) 50 901902]. A
related quinolone, norfloxacin, has been shown to inhibit gyrase
by binding not to the enzyme itself but to regions of ssDNA,
suggesting that gyrase is actually inhibited by a DNAquinolone
complex [PNAS (1985) 82 307311].
[Gyrase-targeted antibiotics: TIM (1998) 6 269275.]
name bearer Syn. NOMENCLATURAL TYPE.
naming of microorganisms See NOMENCLATURE.
NANA N-AcetylNEURAMINIC ACID.
NANB hepatitis NON-ANON-B HEPATITIS.
amplicon
3
1
5
2
5
3
5
6
5
cyclic
phase
8
5
NASBA (nucleic acid sequence-based amplification): isothermal amplification of an RNA target; amplification is carried out at 41 C.
The dashed lines are strands of RNA, the solid lines strands of DNA. For each strand the polarity is indicated by a 3 and/or 5 label.
With clinical specimens, amplification of targets is preceded by treatment of the sample to ensure that target sequences, if present, are made
accessible. Such pre-treatment necessarily includes release of nucleic acid from organisms and heating to denature target RNA; although RNA
is generally single-stranded, intra-strand base-pairing can occur in mRNA and occurs extensively in rRNA. Pre-treatment may also involve
inactivation of inhibitory substances. The following stages are involved in amplification:
1. A strand of RNA showing the target sequence (amplicon) delimited by two, short vertical bars. A primer (primer 1) has bound to the 3
end of the amplicon. The 5 end of this primer is tagged with a short sequence () containing the promoter of an RNA polymerase.
2. The enzyme reverse transcriptase has extended the primer to form a strand of cDNA, thus giving rise to a hybrid RNA:DNA duplex
intermediate.
3. The enzyme RNase H has degraded (removed) the RNA strand. Another primer, primer 2, has bound to the 3 end of the cDNA.
4. Reverse transcriptase (which can also synthesize DNA on a DNA template) has extended primer 2 to form double-stranded cDNA; notice
that the promoter sequence in primer 1 has also become double stranded as primer 2 has been fully extended on the template to form
the complementary strand () of the promoter. Now double-stranded, the promoter is functional; an RNA polymerase () has bound to
the promoter and will synthesize an RNA strand in the direction of the arrow, i.e. in a 5 -to-3 direction.
5. The newly synthesized strand of RNA. Note the strands polarity: it is complementary to the amplicon in the sample RNA (compare 5
with 1).
6. The RNA strand has bound primer 2.
7. Reverse transcriptase has synthesized cDNA on the RNA strand.
8. RNA has been removed by RNase H. Primer 1 has bound to the cDNA.
9. Reverse transcriptase has synthesized a complementary strand of cDNA; note that the 3 end of the template cDNA has also been
extended to form a functional (double-stranded) promoter for the RNA polymerase. RNA polymerase has bound to the promoter and will
(repeatedly) synthesize RNA strands identical to the one shown at stage 5. These strands can participate in the cyclic phase, leading to
high-level amplification of the target. (Continued on page 512.)
511
nasopharyngeal carcinoma
As in other nucleic-acid-amplification methods, products can
be detected by gel electrophoresis and staining. Alternatively,
the amplicons can be monitored by means of MOLECULAR BEACON
PROBES [see e.g. NAR (1998) 26 21502155].
In clinical microbiology, NASBA is useful e.g. for monitoring
the development of transcriptional activity in latent DNA
viruses. For example, by monitoring transcripts of the late genes
of cytomegalovirus (CMV) it is possible to identify patients at
risk for CMV-related disease [JCM (1998) 36 13411346]; a
commercial assay kit for this purpose has been marketed.
[NASBA in diagnostic microbiology, research and other noncommercial applications: RMM (1999) 10 185196.]
[Isothermal nucleic-acid-amplification methods (NASBA,
TMA, SDA): Book ref. 221, pp 126151.]
nasopharyngeal carcinoma (NPC) A carcinoma arising from
the epithelial lining of the post-nasal space. Undifferentiated
NPC is associated with EPSTEINBARR VIRUS (EBV) infection;
the epithelial tumour cells contain multiple copies of EBV
DNA, but chromosomal abnormalities have not been detected
(cf. BURKITTS LYMPHOMA). NPC is generally rare, but occurs
with high incidence among certain ethnic groups, particularly
Cantonese Chinese and Eskimos. Since EBV is ubiquitous,
genetic and/or environmental factors are believed to play a role
in pathogenesis; nitrosamines (present in salted and dried fish
eaten by Cantonese people) and certain components (e.g. phorbol
esters) of Chinese herbal medicines have been implicated as
potentiating factors.
nasopharynx microflora See RESPIRATORY TRACT MICROFLORA.
nasse (protozool.) Syn. CYRTOS.
Nassellarida See RADIOLARIA.
Nassula A genus of freshwater protozoa (subclass HYPOSTOMATIA). Cells: ovoid to elongate, ca. 150200 m in length, completely covered with cilia. Food: e.g. cyanobacteria.
Nassulida See HYPOSTOMATIA.
natamycin Syn. PIMARICIN.
Natronobacterium A genus of halophilic, alkalophilic archaeans
[FEMS Reviews (1986) 39 915].
Natronococcus A genus of halophilic and alkalophilic archaeans
[FEMS Reviews (1986) 39 915].
natto A Japanese food made by fermenting soybeans. Soybeans
are soaked, steam-cooked, wrapped in rice straw, and incubated
at e.g. ca. 40 C for 12 days. Bacillus natto (a strain of
B. subtilis), supplied by the straw or added as a pure-culture
starter, develops and coats the beans with a viscous, sticky
polymer; the product develops a strong persistent flavour. [Book
ref. 8, pp. 520521.]
natural antibodies Immunoglobulins, present in plasma, which
act as antibodies towards antigens with which the body has
apparently not been in immunological contact; they may derive
e.g. from previous or ongoing subclinical infections or from
immunological contact with CROSS-REACTING ANTIGENS.
natural antigen Syn. ANTIGEN (= IMMUNOGEN sense 1).
natural immunological tolerance Syn. SELF TOLERANCE.
natural killer cells See NK CELLS.
Naumanniella A genus of bacteria found e.g. in soil and wellwaters [see e.g. Book ref. 45, pp. 10491059].
Navicula
A genus of pennate DIATOMS in which the cells
are characteristically spindle- or boat-shaped and show gliding
motility. Species occur on mud or other substrates in freshwater,
marine and terrestrial habitats.
NBT Nitroblue TETRAZOLIUM.
NCAM See IMMUNOGLOBULIN SUPERFAMILY.
NCCLS National Committee for Clinical Laboratory Standards
(USA).
Ncd cells See PROTOPLAST FUSION.
NCDO National Collection of Dairy Organisms, Food Research
Institute (Reading), Shinfield, Reading, Berkshire RG2 9AT, UK.
NCIB National Collection of Industrial Bacteria, Torry Research
Station, P.O. Box 31, 135 Abbey Road, Aberdeen AB9 8DG, Scotland, UK.
NCMB National Collection of Marine Bacteria, Torry Research
Station, P.O. Box 31, 135 Abbey Road, Aberdeen AB9 8DG, UK.
NcoI See RESTRICTION ENDONUCLEASE (table).
NCPPB National Collection of Plant Pathogenic Bacteria, Plant
Pathology Laboratory, Hatching Green, Harpenden, UK.
NCS NEOCARZINOSTATIN (q.v.).
NCTC National Collection of Type Cultures, Central Public
Health Laboratory, Colindale Avenue, London NW9 5HT, UK.
NCV NON-CHOLERA VIBRIO.
NCVP Non-O1 Vibrio cholerae pilus (non-cholera-vibrio pilus):
a filamentous cell-surface appendage found in non-O1 strains
of Vibrio cholerae, including many strains of the O139 Bengal
serogroup. (See also CHOLERA.)
NDC Nuclear dehydrogenating clostridia: see GASTROINTESTINAL
TRACT FLORA.
2 -NDG 2 -Nor-2 -deoxyguanosine: see DHPG.
Ndumu virus See ALPHAVIRUS.
NDV NEWCASTLE DISEASE virus.
neamine (neomycin A) An AMINOGLYCOSIDE ANTIBIOTIC whose
molecule contains an aminosugar linked to DEOXYSTREPTAMINE.
Nebraska calf diarrhoea See ROTAVIRUS.
necridium (sacrificial cell) In certain filamentous bacteria (e.g.
certain cyanobacteria, Beggiatoa): a specialized intercalary cell
which, by death and lysis, allows fragmentation of the trichome
and liberation of hormogonia.
necrobacillosis Any of various diseases of man or animals
caused by Fusobacterium necrophorum.
In humans, F. necrophorum can cause e.g. an acute systemic disease characterized by sore throat, submandibular lymphadenopathy, fever with rigors, and subsequently formation of
lung abscesses with consequent pleuritic pain and haemoptysis.
In animals, F. necrophorum may invade the skin or mucous
membranes, usually via damaged tissues, causing necrosis and
sometimes abscess formation. In cattle and lambs the pathogen
may infect via the navel or rumen and then localize e.g. in
the liver. Infections localized to the mouth and larynx (calf
diphtheria) or to the mouth only (necrotic stomatitis) may
also occur. (See also FOOT-ROT.)
NASBA (continued)
The double-stranded cDNA templates in stage 9 are permanent products and are continually transcribed by the RNA polymerase. Operation
of the cyclic phase produces many copies of the amplicon in the form of (i) complementary RNA (the major product), and (ii) cDNA.
In NASBA, amplification involves three enzymes: reverse transcriptase, RNA polymerase and RNase H; in a similar process, TMA, the role of
RNase H is carried out by the reverse transcriptase, so that only two enzymes are used.
Reproduced from Bacteria, 5th edition, Figure 8.25, pages 226227, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN
0471-98880-4) with permission from the publisher.
512
Neisseria
of the needle, and that the length of the needle is regulated by
the invJ gene product [PNAS (2000) 97 1022510230].
[Structure and composition of the Shigella flexneri needle
complex: Mol. Microbiol. (2001) 39 652663.]
Studies on Yersinia enterocolitica suggest that the needle
is formed by polymerization of a 6 kDa protein, and that
polymerization of this protein provides the force necessary
for puncturing the cytoplasmic membrane of a eukaryotic cell
[PNAS (2001) 98 46694674].
Neethling virus See LUMPY SKIN DISEASE.
negative complementation See COMPLEMENTATION TEST.
negative contrast See ELECTRON MICROSCOPY (a).
negative control (of an operon) See OPERON.
negative interference (genetics) See INTERFERENCE (2).
negative Pasteur effect Syn. CUSTERS EFFECT.
negative phase (immunol.) The phase in which the in vivo titre
of a given antibody is reduced following administration of the
homologous antigen due to combination of the antigen with
circulating antibody.
negative-sense genome See VIRUS.
negative staining See STAINING and ELECTRON MICROSCOPY (a).
negative-strand virus A VIRUS (q.v.) with a negative-sense
genome.
Negishi virus See FLAVIVIRIDAE.
Negri bodies Acidophilic, intracytoplasmic INCLUSION BODIES
which develop in cells of the CNS in most cases of human
or animal RABIES. They may occur only in the late stage of the
disease, and are not formed in FIXED VIRUS infections.
negro coffee mosaic virus See POTEXVIRUSES.
neighbour exclusion principle See INTERCALATING AGENT.
NeisserWechsberg leucocidin See staphylococcal a-HAEMOLYSIN.
Neisseria
A genus of aerobic, oxidase-positive, Gram typenegative bacteria (family NEISSERIACEAE) which occur as
parasites or as primary or opportunist pathogens on the mucous
membranes of mammals. Cells: typically cocci, 0.61.0 m in
diameter (which often occur singly, or in pairs with adjacent
sides flattened or concave), but in one species (N. elongata)
the cells are rod-shaped, ca. 0.5 m in width, and often occur
as diplobacilli; the cells tend to resist decolorization in the
Gram stain. Cells may exhibit TWITCHING MOTILITY, and in some
species the FIMBRIAE are associated with pathogenicity. (See
also ANTIGENIC VARIATION and IGA1 PROTEASES.) N. gonorrhoeae
and N. meningitidis are nutritionally fastidious (isolation and
general culture media including e.g. THAYERMARTIN AGAR,
MUELLERHINTON MEDIUM and CHOCOLATE AGAR); the other
species of Neisseria are able to grow on unenriched nutrient
agar. The growth of all species is improved by a high
relative humidity (ca. 50%). Optimum growth temperature:
ca. 3537 C. All strains form CARBONIC ANHYDRASE (cf.
MORAXELLA). Most strains form catalase some strains of
N. elongata are catalase-negative. (See also SUPEROXOL TEST.)
Neisseria spp are highly susceptible to desiccation and to
exposure to direct sunlight. GC%: ca. 46.553.5. Type species:
N. gonorrhoeae.
N. canis. Some strains are haemolytic on rabbit blood; no
acid from glucose or other sugars; nitrate is usually reduced; a
yellow pigment is formed. Strains have been isolated e.g. from
the throats of cats.
N. caviae. See FALSE NEISSERIAE.
N. cinerea. Non-haemolytic; no acid from glucose or other
sugars.
N. cuniculi. See FALSE NEISSERIAE.
Neisseriaceae
N. subflava. Non-haemolytic; acid is usually formed from
glucose and maltose, and sometimes from fructose and sucrose.
Some strains are saline-agglutinable.
Neisseriaceae A family of aerobic, chemoorganotrophic, nonmotile, asporogenous Gram type-negative bacteria which are
typically parasitic and/or pathogenic in warm-blooded hosts.
Most or all strains are oxidase +ve.
The family Neisseriaceae formerly included the genera ACINETOBACTER, KINGELLA, MORAXELLA and NEISSERIA [Book ref. 22,
pp 288309]. The genera Acinetobacter and Moraxella have
been transferred to the family MORAXELLACEAE.
nekton Collectively, the actively motile organisms in a body of
water (e.g. lake, sea). (cf. PLANKTON; see also NEUSTON.)
nelfinavir See ANTIRETROVIRAL AGENTS.
Nelsonian illumination Syn. CRITICAL ILLUMINATION.
nematode-trapping fungi See NEMATOPHAGOUS FUNGI.
nematodesma One of a number of bundles of microtubules
which reinforce the walls of the ciliate CYTOPHARYNX. (cf.
TRICHITE.)
nematophagous fungi A heterogeneous group of fungi which
derive nutrients from nematode worms. Many are predatory,
trapping and killing their prey before invading its tissues, while
others infect and apparently parasitize nematodes; most can also
grow saprotrophically. Nematophagous fungi occur e.g. in soil
and decaying organic matter.
(a) Nematode-trapping fungi. Most fungi in this category
produce various types of specialized trap, generally in response
to the presence of nematodes or of compounds such as certain
peptides or amino acids (collectively termed nemin). These
traps may be simple adhesive knobs (e.g. in Acaulopage
pectospora [CJB (1985) 63 13861390], Dactylaria candida
[CJB (1977) 55 29562970] and Monacrosporium drechsleri ),
relatively undifferentiated adhesive lateral hyphal branches (e.g.
in Triposporina aphanopaga) or adhesive hyphal branches which
branch and anastomose to form two- or three-dimensional
networks (e.g. in Arthrobotrys oligospora, Dactylella cionopaga
[CJB (1984) 62 674679], and some Monacrosporium spp).
[A. oligospora: AvL (1985) 51 385398 (EM study), 399407
(microbodies in trap cells); FEMS Ecol. (1985) 31 1721 (trap
formation in liquid culture).] Non-adhesive hyphal rings are
formed by some species, and these rings may be constricting
(e.g. in Arthrobotrys dactyloides, Dactylaria brochopaga [CJB
(1977) 55 29452955], Dactylella spp) or non-constricting
(e.g. Dactylaria candida which also forms adhesive knobs).
When a nematode enters a ring of the constricting type, the
ring constricts abruptly, trapping and killing the animal; the
mechanism of constriction is unknown, but apparently involves
the rapid swelling of cells of the ring in response to contact
between the inner surface of the ring and the nematode. In the
case of a non-constricting ring, a nematode of appropriate size
may be trapped when it begins to move through the ring but
is too wide to pass right through; in D. candida the rings are
apparently not effective traps [CJB (1977) 55 29562970].
Some fungi (e.g. Stylopage) can trap nematodes without the
formation of specialized structures; when a nematode contacts
a hypha, the hypha secretes at the point of contact an adhesive
which traps the animal.
(b) Fungi endoparasitic in nematodes. Some species (e.g.
Meria coniospora) produce adhesive conidia which adhere to a
nematode and germinate, the hyphae then invading the animal;
after the death of the host, conidiophores emerge from the body.
Harposporium spp produce non-adhesive conidia, and a nematode becomes infected by ingestion of these conidia. Certain
Nephroma
chytridiomycetes (e.g. Catenaria), oomycetes (e.g. Nematophthora gynophila) and zygomycetes (e.g. Gonimochaete pyriforme [EM study: CJB (1985) 63 23262331]) can infect and
parasitize nematodes; N. gynophila can apparently play a role
in the control of the cereal cyst nematode, Heterodera avenae
[Nematol. (1980) 26 5768].
Nematophthora See NEMATOPHAGOUS FUNGI.
Nematospora A genus of fungi (family METSCHNIKOWIACEAE)
in which multilateral budding occurs; a well-developed pseudomycelium is usually formed, and true mycelium may be
formed. Ascospores: fusiform with a whip-like appendage at
one end, usually 8 per ascus. Species occur mainly as parasites
and pathogens of plants (see e.g. STIGMATOMYCOSIS). [Book ref.
100, pp. 285288.]
Nematosporaceae Syn. METSCHNIKOWIACEAE.
Nematostelium See PROTOSTELIOMYCETES.
nemin See NEMATOPHAGOUS FUNGI.
neoantigen An antigen formed in vivo by the combination of
a protein with an exogenous substance. (See also CONTACT
SENSITIVITY.)
Neocallimastix A genus of anaerobic fungi found in the RUMEN;
species include N. patriciarum [TBMS (1986) 86 178181,
103109] and N. frontalis. N. frontalis forms multiflagellate
zoospores [ultrastructure: CJB (1983) 61 295307] and produces an extracellular cellulase which is more effective than any
other known cellulases in solubilizing the extensively hydrogenbonded cellulose in cotton fibres [FEMS (1986) 34 3740]. It
has been proposed that Neocallimastix be placed in an amended
class CHYTRIDIOMYCETES. [Mitosis in and phylogeny of the genus
Neocallimastix: CJB (1985) 63 15951604.]
neocarzinostatin (NCS) An antitumour agent, produced by
Streptomyces carzinostaticus, which consists of an acidic 109amino-acid protein (containing two disulphide bonds) linked
non-covalently to a complex, highly labile, non-protein chromophore which is responsible for the activity of the drug. In
vitro, NCS interacts with DNA (its chromophore behaving as an
INTERCALATING AGENT), causing single-stranded breaks in which
the 3 and 5 ends generally bear 3 -phosphate and 5 -aldehyde
groups, respectively; strand breakage occurs mainly at thymidine
and deoxyadenosine residues and requires the presence of a thiol
and O2 as cofactors. NCS-induced strand breakage in intact cells
appears to occur by a reaction similar to that in vitro [Biochem.
(1987) 26 384390]. NCS can also cause e.g. release of free
bases (particularly thymine and adenine) from the DNA.
Neodiprion sertifer NPV See BACULOVIRIDAE.
neogregarines See GREGARINASINA.
neomycin Either of two related AMINOGLYCOSIDE ANTIBIOTICS
(neomycins B, C) produced by Streptomyces fradiae; the drug
used clinically consists mainly of neomycin B with some
neomycin C. (cf. NEAMINE.)
neonatal calf diarrhoea coronavirus See CORONAVIRIDAE.
neonatal herpes See HERPES SIMPLEX.
neoplasia Progressive, uncontrolled cell division which, if the
progeny cells remain localized (at least initially), results in
the formation of an abnormal growth (tumour, neoplasm). (cf.
HYPERPLASIA.) In man or animals, a neoplasm may be BENIGN or
MALIGNANT (sense 2). (See also CANCER; cf. LEUKAEMIA.)
neoplasm See NEOPLASIA.
Neorickettsia A genus of Gram-negative bacteria of the tribe
EHRLICHIEAE. Cells: coccoid, often pleomorphic, non-motile,
maximum dimension ca. 0.5 m. Growth occurs intracytoplasmically in lymphoid cells of canine animals. Growth does not
occur in cell-free media. Type species: N. helminthoeca.
Nephroselmis
of amplification (20 cycles) the annealing temperature was lowered to 45 C permitting binding of the inner primers and leading to the formation of second-phase amplicons. Detection of the
second-phase amplicons involved pre-labelling of inner primers.
One type of primer was 5 -biotinylated while the other was 5 labelled with DIGOXIGENIN so that the double-stranded amplicon was labelled with both compounds. By means of the biotin
tag, amplicons were captured on an AVIDIN-coated microtitre
plate; an antidigoxigeninalkaline phosphatase conjugate was
used to label the amplicon (by digoxigeninantidigoxigenin
binding), and the label (enzyme) was detected by addition of
a reagent (p-nitrophenylphosphate) and monitoring colorimetrically at 405 nm for the enzymic cleavage products.
Other examples of nPCR include detection of Mycobacterium malmoense [JCM (1999) 37 14541458], and nested
duplex PCR for the detection of Bordetella pertussis and
B. parapertussis [JCM (1999) 37 606610].
net blotch A CEREAL DISEASE, caused by Pyrenophora teres,
which affects mainly winter barley. Pale, yellowish blotches,
later turning brown, appear on leaves in the autumn; the brown
lesions, which have a net-like appearance, may coalesce to
form longitudinal stripes. (See also FLUTRIAFOL, GUAZATINE,
PROCHLORAZ, PROPICONAZOLE.)
net plasmodium See LABYRINTHULAS.
net slime moulds See LABYRINTHULAS.
netilmicin An AMINOGLYCOSIDE ANTIBIOTIC.
netropsin A basic oligopeptide ANTIBIOTIC (isolated from Streptomyces netropsis) containing two N-methylpyrrole rings; the
functionally similar distamycin A contains three such rings. Both
netropsin and distamycin bind specifically and avidly to BDNA, with a strong preference for AT-rich regions [DNAdrug
specificity: PNAS (1985) 82 13761380]; the drug appears to
bind (non-intercalatively) in the minor groove (see DNA). Both
drugs show antimicrobial and antitumour activity (apparently by
inhibiting synthesis of RNA and DNA) and inhibit the development of DNA viruses, but they are too toxic for clinical use.
Low concentrations of netropsin have been reported to inhibit
sporulation without affecting growth in Bacillus subtilis [CJM
(1980) 26 420426].
Neubergs fermentations Neubergs 1st form of fermentation
is the ALCOHOLIC FERMENTATION as normally carried out by yeasts
such as Saccharomyces. Neubergs 2nd form of fermentation
(= glycerol fermentation, sulphite fermentation) refers to
the alcoholic fermentation perturbed by the presence of sodium
bisulphite (NaHSO3 ). Bisulphite forms an addition compound
with acetaldehyde, preventing its reduction (by NADH) to
ethanol; NADH (from the EMP pathway) instead reduces
dihydroxyacetone phosphate to glycerol-3-phosphate which
is dephosphorylated to GLYCEROL. Neubergs 3rd form of
fermentation refers to the alcoholic fermentation perturbed by
imposed alkalinity; the end products are glycerol, ethanol and
acetic acid.
Neufchatel cheese See CHEESE-MAKING.
Neufeld quellung phenomenon See QUELLUNG PHENOMENON.
neuraminic acid A C9 -compound (5-amino-3,5-dideoxy-D-glycero-D-galactononulosonic acid) derived from mannosamine
and pyruvate; N-acetyl and O-acetyl derivatives (e.g. Nacetylneuraminic acid, NANA) are called sialic acids. Sialic
acids occur widely in animal tissues and fluids e.g. in glycolipids, mucopolysaccharides and mucoproteins in mucous
secretions, serum, brain glycolipids (gangliosides), milk (Nacetylneuraminyllactose), etc. Terminal sialic acid residues in
glycoprotein or glycolipid cell membrane components serve as
Newcombe experiment
neutropenic enterocolitis (ileocaecal syndrome) (med.) A syndrome characterized by neutropenia (a diminished number of
circulating neutrophils) and ulceration, haemorrhage and necrosis of the distal ileum or caecum; Clostridium septicum may play
a major causative role in the symptoms.
neutrophil An amoeboid, phagocytic PMN (q.v.) responsive to
chemotactic stimuli often the major type of cell involved early
in acute INFLAMMATION. Neutrophils contain many enzymes (e.g.
LYSOZYME, MYELOPEROXIDASE) (see also BPI PROTEIN, LACTOFERRIN). Stimulation (e.g. by opsonized bacteria or concanavalin A)
leads to a respiratory burst (metabolic burst) of increased oxygen consumption (over several minutes) starting within seconds
of stimulation; much of the oxygen may be used to form SUPEROXIDE radicals (see PHAGOCYTOSIS). (cf. MACROPHAGE.) (See also
CALPROTECTIN.)
neutrophile An organism which has an optimum growth pH
within the pH range 68. (cf. ACIDOPHILE and ALKALOPHILE.)
nevirapine See ANTIRETROVIRAL AGENTS and AIDS.
Nevskia A poorly characterized genus of aquatic bacteria [see
e.g. Book ref. 45, pp. 520523].
new combination In NOMENCLATURE: syn. COMB. NOV. (q.v.).
new variant CJD See CREUTZFELDTJAKOB DISEASE.
New World arenaviruses See ARENAVIRIDAE.
Newcastle disease (avian pneumoencephalitis; Ranikhet disease)
A highly infectious POULTRY DISEASE caused by a PARAMYXOVIRUS. Chickens, turkeys and pheasants may be affected, and
mild infections have been reported in ducks, geese and pigeons.
Transmission may occur by droplet inhalation or by ingestion
of contaminated water or food (e.g. food contaminated with
infected pigeon droppings [VR (1984) 115 601602]). Incubation period: ca. 412 days. Symptoms: variable, but commonly
include e.g. loss of appetite, diarrhoea, laboured breathing, discharge from eyes, nostrils and mouth, often followed by neurological signs (drowsiness, weakness, paralysis). Mortality rates
vary from 0 to ca. 100%. Lab. diagnosis: identification of the
virus; an HAI test. Control: slaughter of infected flocks; vaccination using either live or inactivated vaccines.
The Newcastle disease virus has been reported to cause
conjunctivitis in man.
Newcombe experiment An experiment by which Newcombe (in
1949) demonstrated that the apparent adaptation of a bacterial
population to an altered environment involves the selection of
pre-existing mutants.
Nutrient agar plates are each spread with the same quantity of
inoculum from a single culture of phage-sensitive bacteria. The
plates are incubated for a few hours, during which time each
viable cell gives rise to a clone. The plates are then divided
into two groups. In group A, the bacterial growth on each plate
is redistributed (with a sterile glass spreader) so that the cells
of each clone are dispersed over the agar surface. Group B
plates are left undisturbed. All plates are then sprayed with a
suspension of virulent phage and re-incubated. All the sensitive
bacteria lyse; thus, colonies which subsequently develop on any
plate must have arisen from cells which were, or had become,
resistant to phage.
If phage-resistant bacteria developed adaptively, resistant cells
would be formed only after exposure of phage; the redistribution
of growth in group A plates would therefore not influence the
subsequent development of resistant cells, and similar numbers
of resistant cells and hence colonies should appear on all
the plates. If, however, phage-resistant cells arose spontaneously
before exposure to phage, each resistant (mutant) cell would
form a discrete clone of resistant cells; subsequent redistribution
nexin
nicotinic acid (niacin) Pyridine 3-carboxylic acid; the corresponding amide, nicotinamide, is a component of the important
coenzymes NAD (q.v.) and NADP. Niacin may be biosynthesized
(via quinolinic acid) from aspartate and dihydroxyacetone phosphate (e.g. in many bacteria, and in Saccharomyces cerevisiae
growing under anaerobic conditions), or from tryptophan (e.g.
in Xanthomonas spp and in most fungi including S. cerevisiae
growing under aerobic conditions). Organisms auxotrophic for
niacin or nicotinamide include e.g. Lactobacillus spp (used in
the BIOASSAY of niacin), Morganella and Proteus spp (but not
Providencia), Bordetella pertussis, some yeasts and fungi (e.g.
Mucor rouxii requires niacin under anaerobic conditions but not
under aerobic conditions), and certain protozoa (e.g. Tetrahymena pyriformis, coccidia). (See also NIACIN TEST; V FACTOR;
VITAMIN.)
niddamycin See MACROLIDE ANTIBIOTICS.
Nidula See NIDULARIALES.
Nidulariales An order of humicolous, lignicolous or coprophilous
fungi (class GASTEROMYCETES) characterized by a type of basidiocarp in which the GLEBA occurs in several parts, each part
contained within a closed chamber (peridiole) which is physically separate from the other chambers; in some species each
peridiole is attached to the inside of the (typically cup-shaped or
funnel-shaped) peridium by a complex, extensible structure. The
appearance of peridioles at the bottom of the peridium (which
is open at maturity) has earned these fungi the name birds
nest fungi. Genera include Crucibulum, CYATHUS, Mycocalia
and Nidula.
nif genes Genes whose expression is necessary for NITROGEN FIXATION. In Klebsiella pneumoniae there are at least 17 nif genes
clustered (close to the his operon) in 8 contiguous transcriptional
units (nifJ, nifHDK, nifY, nifENX, nifUSVM, nifF, nifLA, and
nifBQ) spanning ca. 23 kb on the chromosome. Genes nifHDK
are structural genes for NITROGENASE: nifD and nifK specify the
two subunits of the MoFe protein (Kp1), nifH specifies the
subunit of the Fe protein (Kp2). The nifJ product is the pyruvate:flavodoxin oxidoreductase which transfers electrons from
pyruvate to the flavodoxin (nifF product) that reduces the Fe
protein of nitrogenase. The nifB, nifE, nifN and nifV genes all
appear to be involved in the synthesis of the FeMo cofactor; nifQ
appears to be involved in molybdate uptake; nifM, nifS and nifU
may be involved in the processing of nitrogenase components;
nifL and nifA are concerned with nif gene expression.
Expression of nif genes in K. pneumoniae is regulated at the
transcriptional level and is repressed e.g. by alternative sources
of nitrogen, by high oxygen levels, etc. The nifA gene specifies
an activator of transcription which is necessary for the expression
of most nif genes. The nifL gene specifies a negative regulator
which represses transcription in the presence of e.g. amino acids,
low levels of NH4 + , and oxygen; it appears not to interact
directly with DNA but may complex with and inactivate the
NifA protein. Transcription of nif genes is regulated by the
availability of combined nitrogen and is subject to control by
the NTR GENES.
The nif genes of other bacteria are generally less well
characterized: Azotobacter appears to have additional copies of
nifH; in Bradyrhizobium strains nifH is separated from nifDK;
Rhodopseudomonas capsulata has multiple copies of nifHDK,
while its other nif genes are apparently more widely dispersed on
the chromosome than are those of K. pneumoniae. In Rhizobium
spp nif genes are located on the Sym plasmid (see entry ROOT
NODULES).
In most nitrogen-fixing CYANOBACTERIA, nif genes are
expressed only in HETEROCYSTS. In vegetative cells of e.g.
nitrate respiration
[Synergistic action of nisin and CO2 against Listeria monocytogenes: AEM (2000) 66 769774. Bioassay for nisin in food:
AEM (2003) 69 42144218.]
Nitella See CHAROPHYTES.
nitrapyrin (N-Serve) 2-Chloro-6-(trichloromethyl)pyridine, a NITRIFICATION INHIBITOR.
nitratase Syn. nitrate reductase.
nitrate broth Nutrient broth (or peptone water) containing KNO3
(0.10.2% w/v).
nitrate reductase See ASSIMILATORY NITRATE REDUCTION; DENITRIFICATION; NITRATE RESPIRATION.
nitrate reduction See ASSIMILATORY NITRATE REDUCTION and DISSIMILATORY NITRATE REDUCTION.
nitrate reduction test (nitrate test) A test used to indicate
whether or not a given bacterial strain can reduce nitrate; the
medium and test conditions used depend on the particular organism being examined. For many bacteria (including enterobacteria
and pseudomonads, but excluding e.g. Mycobacterium spp) the
organism is cultured for 25 days in NITRATE BROTH. The culture
is then tested for the presence of nitrite by adding 0.5 ml reagent
A (0.8% w/v sulphanilic acid in 5 N acetic acid) followed by
0.5 ml reagent B (0.6% w/v N,N-dimethyl-a-naphthylamine
in 5 N acetic acid); if present, nitrite reacts with sulphanilic acid
to form a diazonium salt which, with the naphthylamine, forms
a soluble red azo dye. The absence of coloration could mean
that either (a) nitrate has not been reduced, or (b) the nitrite has
itself been reduced. To resolve this question a trace of zinc dust
is added; if nitrate is present it is reduced (by the zinc dust) to
nitrite (which gives a red coloration) the absence of coloration
indicating possibility (b).
For Mycobacterium spp, a small loopful of growth is dispersed in 0.02 M phosphate buffer (pH 7.0) containing 0.01 M
NaNO3 , and the suspension is incubated (37 C/2hours). To the
suspension is then added 1 drop of HCl (concentrated HCl:water
mixed 1:1 v/v) followed by 2 drops of sulphanilamide solution (0.2% aqueous) and 2 drops of N-naphthylethylenediamine
dihydrochloride (0.1% aqueous); pink or red coloration indicates
reduction of nitrate to nitrite. If no colour develops, the addition
of zinc dust causes a red coloration if the medium still contains nitrate and fails to do so if the nitrate had been reduced
beyond nitrite.
nitrate respiration ANAEROBIC RESPIRATION in which, typically,
nitrate (as terminal electron acceptor) is reduced to nitrite in a
reaction catalysed by an enzyme (dissimilatory nitrate reductase)
located at the end of an ELECTRON TRANSPORT CHAIN; this
reaction, which is equivalent to the first stage of DENITRIFICATION,
generates proton motive force (pmf: see CHEMIOSMOSIS) which
can be used e.g. for ATP synthesis. (cf. DISSIMILATORY NITRATE
REDUCTION.) In some organisms the nitrite is excreted, but in
others it can be reduced to ammonia. In nitrate respiration the
energy yield is less than that obtainable with oxygen as electron
acceptor.
In some bacteria (including e.g. Escherichia coli ) nitrate can
be used for the anaerobic oxidation of e.g. NADH, succinate
and/or formate pmf being generated in each case; the resulting
nitrite inhibits aconitase and fumarase, thus inhibiting the TCA
cycle [Appendix II(a)].
In e.g. Escherichia coli a soluble (assimilatory) nitrite reductase can catalyse the anaerobic reduction of nitrite to ammonia in
a reaction coupled to the oxidation of NADH. This reaction does
not, in itself, yield energy; however, by regenerating NAD+ from
NADH (produced during the metabolism of e.g. glucose) it tends
to prevent the (energetically wasteful) synthesis of ethanol see
Anabaena, the nifH and nifD genes are contiguous, but nifK
is separated from nifD by ca. 11 kb. It has been shown that,
late in heterocyst differentiation, the DNA undergoes certain
rearrangements, including the excision and circularization of the
11-kb segment between nifD and nifK; this results in the fusion
of nifK with nifHD and allows coordination of transcription of
the nifHDK genes.
[nif and associated genes in Acetobacter diazotrophicus: JB
(2000) 182 70887091.]
nifuratel See NITROFURANS.
nifuroxime See NITROFURANS.
nifurprazine See NITROFURANS.
nigeran (mycodextran) A linear a-D-glucan in which glucopyranose residues are linked by alternating (1 3)-a- and (1
4)-a-glycosidic linkages; it is soluble in hot water. Nigeran
occurs in the hyphal walls of Aspergillus spp (but not in
A. nidulans, which contains PSEUDONIGERAN) and Penicillium
spp. [Nigeran as a phylogenetic marker: Mycol. (1978) 70
12011211.]
nigericin A linear MACROTETRALIDE antibiotic which can act as
a mobile carrier IONOPHORE for the transport of monovalent
cations K+ or Rb+ (or, to a lesser extent, e.g. Na+ ). In order to
transport an ion the nigericin molecule loses a proton and binds
the ion, and the (electrically neutral) nigericinion complex
diffuses across the membrane; since nigericin can also cross the
membrane in a protonated state, it can bring about the exchange
of H+ for K+ (see ELECTRONEUTRAL TRANSPORT). Nigericin is
used e.g. to alter a membrane pH gradient (see CHEMIOSMOSIS).
nigerose a-D-Glucopyranosyl-(1 3)-D-glucopyranose.
nigrosin A black composite indulin-based DYE used e.g. for
negative STAINING.
nikA gene See CONJUGATION (1b)(i).
nikkomycins A group of antibiotics which closely resemble
POLYOXINS both in structure and in mode of action; nikkomycins
have a wider spectrum of activity than polyoxins, being more
active e.g. against the yeast forms of Mucor rouxii and Candida
albicans.
Nikolsky sign Wrinkling of the skin (evident on gentle stroking)
due to separation of the outer epidermis from the basal layer.
(See also EPIDERMOLYTIC TOXIN.)
Nile blue A (Nile blue sulphate) A blue basic oxazine DYE used
e.g. in VITAL STAINING and as a lipid stain. In aqueous solution
some of the dye is spontaneously oxidized to the phenoxazone
LYSOCHROME Nile red (soluble in aqueous Nile blue A); this
allochromatic mixture stains fatty acids and phospholipids blue,
and neutral lipids red. Nile blue A can be used as a fluorescent
stain for poly-b-hydroxybutyrate [AEM (1982) 44 238241];
Nile red is useful as a vital stain for intracellular lipid droplets,
being strongly fluorescent only in a hydrophobic environment
[JBC (1985) 100 965973].
Nile red See NILE BLUE A.
nisin A low-MWt LANTIBIOTIC produced by strains of Lactococcus; genes for nisin synthesis appear to be plasmid-borne.
[Nisin (review): AAM (1981) 27 85123.] Nisin is bactericidal
against Gram-positive bacteria, and has some sporicidal activity;
it is both heat-stable and acid-stable, but stability and solubility
decrease with increasing pH, and nisin is inactivated by certain
proteases (e.g. chymotrypsin). Nisin is not used clinically; it is
employed as a food PRESERVATIVE, generally in conjunction with
heat treatment, in e.g. milk and DAIRY PRODUCTS (in which it
occurs naturally) and certain canned vegetables. Canned, lowacid foods in which nisin is used must still receive adequate heat
treatment because Clostridium botulinum is relatively resistant
to nisin. (cf. DIPLOCOCCIN and SUBTILIN.)
519
nitrate test
aquatic environments, and in the upper (aerobic) region of some
sediments. (See also SEWAGE TREATMENT.) Nitrification is carried
out by autotrophic bacteria of the family NITROBACTERACEAE
and by many heterotrophic organisms, including some fungi. It
has been generally supposed that only the autotrophic nitrifying
bacteria carry out nitrification to an ecologically significant
extent; however, while this appears to be the case e.g. in the
sediments of a Scottish estuary [JGM (1984) 130 23012308],
the potential for heterotrophic nitrification was found to be
greater than that for autotrophic nitrification in a Californian
forest soil [AEM (1984) 48 802806].
Autotrophic nitrification occurs in two stages, each stage being
carried out by one of the two categories of nitrifying bacteria.
(a) Ammonia to nitrite (nitrosofication). Ammonia is initially
oxidized to hydroxylamine (NH2 OH) in a MONOOXYGENASEdependent, non-energy-yielding reaction; NH2 OH is then oxidized to nitrite by an enzyme complex, electrons being transferred to molecular oxygen with concomitant oxidative phosphorylation. (b) Nitrite to nitrate. The oxidation of nitrite to
nitrate provides energy by oxidative phosphorylation: in at least
some nitrite-oxidizing bacteria NO2 is oxidized in the reaction: NO2 + H2 O NO3 + 2H+ + 2e ; the electrons are
believed to be transferred to cytochrome (cyt) a1 which in turn
transfers them via cyt aa3 to molecular oxygen, 1ATP being
formed for each pair of electrons transferred.
In the nitrite-oxidizing bacteria (and probably also in NH4 +
oxidizers) pyridine nucleotide coenzymes are reduced by
reversed electron transport. In at least some nitrite oxidizers,
electrons appear to pass from cyt a1 , via cyts c and b, to a
flavoprotein and thence to the pyridine nucleotides; this process is highly energy-dependent, so that nitrifying bacteria need
large quantities of NO2 to sustain their relatively slow rates of
growth.
Agriculturally, nitrification can be disadvantageous under
certain conditions: NO3 is readily leached from the topsoil
by rain thereby becoming unavailable as a source of crop
nitrogen. (By contrast, owing to its charge, NH4 + is more
strongly adsorbed to soil particles and is relatively immobile in
top-soils.) Nevertheless, when e.g. the crops nitrogen demand
is high and the rainfall (and hence risk of leaching) is likely to
be low, rapid nitrification may actually be desirable since (a)
optimal growth in many or most plants appears to occur only
when both NH4 + and NO3 are available, and (b) NH4 + may
be assimilated (in preference to NO3 ) by soil microorganisms
so that, in the absence of nitrification, much of the available
soil nitrogen may be lost to crops as a consequence of being
immobilized in microbial biomass. However, when e.g. the risk
of leaching is high, the use of NITRIFICATION INHIBITORS can be
advantageous; these agents have a temporary effect (they are
gradually lost by evaporation and/or decomposition), and they
not only benefit soil fertility but also reduce the pollution of
groundwater by nitrate. (See also NITROGEN CYCLE.)
nitrification inhibitors Agents which retard or block NITRIFICATION; nitrification inhibitors appear to be typically bacteriostatic under field conditions. The agriculturally important agents
inhibit microbial oxidation of ammonia and may also inhibit
the oxidation of nitrite though nitrite oxidation is generally
much less sensitive to these agents; agents which block only
nitrite oxidation cannot be used since they could cause accumulation of (phytotoxic) nitrite ions. Commercial nitrification
inhibitors some of which also have useful antifungal properties include e.g. DICYANDIAMIDE, ETRIDIAZOLE and NITRAPYRIN.
(See also BARBAN and CARBON DISULPHIDE.) [Review: Book ref.
121, pp. 3343.]
nitrogen fixation
In laboratory studies, acetylene has been used to block
ammonia oxidation, and chlorate to block nitrite oxidation, in
autotrophic nitrifiers [AEM (1984) 48 802806].
nitrifying bacteria See NITROBACTERACEAE.
nitriloacetic acid See NTA.
nitrite (a) (as a food additive and preservative) See e.g. CURING
(sense 1).
(b) (in the environment) See NITROGEN CYCLE.
nitrite reductase See ASSIMILATORY NITRATE REDUCTION; DENITRIFICATION; NITRATE RESPIRATION.
nitrite respiration See NITRATE RESPIRATION.
Nitrobacter A genus of Gram-negative bacteria of the NITROBACTERACEAE; strains occur in soils and in freshwater and marine
habitats. Cells of the type species, N. winogradskyi, are rods
ca. 0.60.8 1.02.0 m; they are commonly non-motile but
may have a single polar flagellum. Peripherally arranged
cytomembranes form a cap at one pole of the cell. The cells
reproduce by budding. Some strains are obligate chemolithoautotrophs which obtain energy by oxidizing nitrite to nitrate;
other strains are facultatively chemoorganoheterotrophic. Storage compounds include PHB. Growth occurs optimally at
ca. 2530 C and at a pH of ca. 7.58.0. GC%: ca. 61. (See
also CARBOXYSOMES.)
Nitrobacteraceae (nitrifying bacteria) A family of Gramnegative, asporogenous, obligately aerobic bacteria which occur
e.g. in soil and in freshwater and marine habitats; the organisms obtain energy by the oxidation of ammonia or nitrite (see
NITRIFICATION), and all except some strains of Nitrobacter winogradskyi are obligate chemolithoautotrophs. The family includes
coccoid, rod-shaped, spiral and lobate bacteria. Cells may be
non-motile or may have polar, subpolar or peritrichous flagella. The cells of many species contain characteristic cytomembranes. Most species divide by binary fission; budding occurs
in Nitrobacter winogradskyi. Species which oxidize ammonia
to nitrite are placed in the following genera: NITROSOCOCCUS,
NITROSOLOBUS, NITROSOMONAS, NITROSOSPIRA and NITROSOVIBRIO;
nitrite-oxidizing species are placed in the genera NITROBACTER,
NITROCOCCUS and NITROSPINA.
nitroblue tetrazolium See TETRAZOLIUM.
nitrocefin A chromogenic cephalosporin used to test for bLACTAMASES; when cleaved by a b-lactamase it changes from
yellow to red. (See also PADAC.)
Nitrococcus
A genus of Gram-negative marine bacteria of
the NITROBACTERACEAE. Cells of the type species, N. mobilis,
are coccoid, ca. 1.51.8 m diameter, each having one or
two subpolar flagella; the cells contain tubular cytomembranes
arranged randomly in the cytoplasm. The cells reproduce by
binary fission. GC%: ca. 61.
nitrofurans A family of synthetic ANTIBIOTICS which are derivatives of 2-substituted 5-nitrofurans; they are active against many
Gram-positive and Gram-negative bacteria, certain fungi, and
some protozoa. Some nitrofurans are used as chemotherapeutic agents, but many are known to be mutagenic/oncogenic.
The antibacterial activity of a nitrofuran depends on the (stepwise) intracellular reduction of the nitro group, the intermediate(s) formed being able to cause strand breakage in DNA.
(cf. NITROIMIDAZOLES.) In e.g. Escherichia coli, the reduction
of a nitrofuran involves NADH-linked nitrofuran reductase 1
(NR1) and NADPH-linked nitrofuran reductase 2 (NR2);
mutants lacking NR1 exhibit high-level resistance to nitrofurans.
(Little is known about plasmid-encoded resistance to nitrofurans;
if it exists, the incidence appears to be negligible.) [Resistance
to nitrofurans: Book ref. 160, pp. 317344.] Examples of nitrofurans:
Furaltadone is used e.g. against colibacillosis and salmonellosis in pigs and cattle. (See also PULLORUM DISEASE.)
Furazolidone (furoxone) has been used e.g. against bacillary
dysentery and Salmonella infections in man, and is used e.g.
in the treatment of human GIARDIASIS and certain diseases of
animals (e.g. BLACKHEAD).
Furylfuramide (AF-2 ) is an oncogenic nitrofuran once used
as a food preservative in Japan.
Nifuratel has been used e.g. against vaginal trichomoniasis.
Nifuroxime has been used, topically, as an antifungal agent,
being active against e.g. Candida albicans; it has also been used
(in conjunction with furazolidone) against vaginal trichomoniasis.
Nifurprazine is used as a topical, broad-spectrum antibacterial
agent.
Nitrofurantoin (furadantin) is the most widely-used nitrofuran. It is used as a broad-spectrum antibacterial agent against
infections of the (human) urinary tract; many strains of Pseudomonas aeruginosa are resistant, and resistant strains of e.g.
Proteus also occur.
Nitrofurazone (furacin) is used, rarely, for the topical treatment of e.g. infected wounds.
nitrofurantoin See NITROFURANS.
nitrofurazone See NITROFURANS.
nitrogen cycle In nature: the cyclical interconversion of nitrogen and its compounds by living organisms and non-biological
processes. The major microbial conversions are shown on
page 522. (See also AMMONIA ASSIMILATION, AMMONIFICATION,
ASSIMILATORY NITRATE REDUCTION, DENITRIFICATION, DISSIMILATORY NITRATE REDUCTION, DISSIMILATORY REDUCTION OF NITRATE
TO AMMONIA, NITRATE RESPIRATION, NITRIFICATION, NITROGEN FIXATION.) (cf. CARBON CYCLE and SULPHUR CYCLE.)
nitrogen fixation (dinitrogen fixation) The reduction of gaseous
nitrogen (dinitrogen, N2 ) to ammonia. (See also NITROGEN
CYCLE.)
Biological nitrogen fixation is carried out only by certain
prokaryotes; these nitrogen-fixing organisms are called diazotrophs. The diazotrophs include various cyanobacteria (e.g.
Anabaena, Nostoc, Plectonema, Trichodesmium); certain species
of Bacillus and Clostridium; Azospirillum; Klebsiella pneumoniae (some strains); members of the Azotobacteriaceae, Methylococcaceae, Rhizobiaceae and Rhodospirillales; and certain
species of the Archaea.
That plants are unable to fix nitrogen is interesting in
that, during evolution, plants are believed to have incorporated
prokaryotes as organelles (e.g. mitochondria). However, during
that period of evolution, prokaryotes may not have yet developed
nitrogen-fixing ability and, moreover, plants may not have been
subjected to sufficient selection pressure [PTRSLB (1992) 338
409416].
The free-living diazotrophs occur e.g. in soil and water,
while a number of diazotrophs form symbiotic associations
with other organisms (which benefit from a supply of fixed
nitrogen). AZOSPIRILLUM fixes nitrogen in the RHIZOSPHERE of
various plants, including some important crop plants. Certain
species of AZOTOBACTER fix nitrogen in association with the roots
of a grass, Paspalum notatum, and the surface of the green
seaweed Codium. Clostridium spp are found in waterlogged
(anaerobic) soils, and may also fix nitrogen in the intestines
of man and other animals.
Frankia spp form symbiotic associations with certain
non-leguminous plants (see ACTINORRHIZA), while Rhizobium/Bradyrhizobium spp are found in leguminous ROOT NODULES and STEM NODULES.
521
nitrogen fixation
NO3
nitra
te r
e
sp
ira
ti o
ct
io
du
tr
ni
o
a ti
ifi c
Nitrobacter
Nitrococcus
ss
im
il a
to
ry
te
tra
ni
Clostridium spp
Escherichia coli
re
Bacillus licheniformis
Pseudomonas stutzeri
Thiobacillus denitrificans
NO2
denit
r i fi
cat
ion
N2
on
n it
r ifi
c at
io n
on
p ir
a ti
es
)r
it e
re
du
ct
io
n
io n
Nitrosococcus
Nitrosomonas
il a t
tra
te
nitrogen fixati
ni
sim
ry
as
to
organic
matter
Some cyanobacteria
Azotobacteraceae
Rhizobium
ia
il a
ica
tio
on
si
am
mo
n if
as
NO2
NH3
am
t
itra
(n
it r
NH4
NITROGEN CYCLE microbial aspects, with examples of organisms. (For cross-references see entry NITROGEN CYCLE.) Not shown is the activity
of ANAMMOX BACTERIA (q.v.).
Reproduced from Bacteria 5th edition, Figure 10.2, page 258, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
Nitrogen fixation is catalysed by the enzyme complex NITROThe reaction requires a strong reducing agent (source
of electrons) and consumes 1216 molecules of ATP per
molecule of nitrogen fixed; electrons from a source such as
hydrogen or NADPH are transferred e.g. to a FERREDOXIN or
FLAVODOXIN and thence to nitrogenase. (For in vitro work, the
artificial reductant dithionite can be used.)
In some diazotrophs (e.g. Bacillus polymyxa, Clostridium pasteurianum, Klebsiella pneumoniae, some cyanobacteria) reducing power and ATP can both be obtained from pyruvate.
Reducing power is provided by the oxidative decarboxylation
of pyruvate to acetyl-CoA (catalysed by the enzyme pyruvate:flavodoxin oxidoreductase); the acetyl-CoA is converted to
acetyl phosphate from which phosphate can be transferred to
ADP in a substrate-level phosphorylation.
The ammonia produced by nitrogen fixation may be assimilated e.g. via the GOGAT pathway (see AMMONIA ASSIMILATION).
Nitrogenase is highly sensitive to oxygen, and many diazotrophs (e.g. clostridia) fix nitrogen anaerobically or microaerobically. In some cyanobacteria the process is carried out within
specialized cells (see HETEROCYST). Certain diazotrophs have
specific mechanisms for protecting nitrogenase during aerobic
nitrogen fixation; for example, rhizobium bacteroids in ROOT
GENASE.
522
Nitrosomonas
are protected by LEGHAEMOGLOBIN. (See also TRIStrains of Azotobacter and possibly Gloeothece
[JGM (1984) 130 495503] exhibit oxygen-scavenging respiratory protection: they show high rates of respiration in the
presence of high levels of oxygen, their branched respiratory
chains being poorly coupled to ATP synthesis; respiration thus
serves primarily to consume oxygen. In those organisms which
have an uptake hydrogenase (see NITROGENASE), the transfer
of electrons from hydrogen via an electron transport chain to
oxygen (as terminal electron acceptor) may also help to protect
nitrogenase from oxygen. In unicellular, aerobic, nitrogen-fixing
cyanobacteria of the genus Cyanothece, nitrogen fixation was
found to occur only in the dark period during alternating 12-hour
light/dark cycles, but was continuous during 24-hour illumination; nitrogen fixation during the dark period would avoid exposure to the oxygen evolved by photosynthesis, but continuous
fixation during continual illumination requires additional explanation and may involve the inclusion granules that develop
under nitrogen-fixing conditions [JB (1993) 175 12841292].
[Cyanobacterial nitrogen fixation (oxygen relationships): MR
(1992) 56 340373. Nitrogen fixation by non-heterocystous
cyanobacteria: FEMS Reviews (1997) 19 139185.]
nitrogen mustards Highly reactive bifunctional ALKYLATING
AGENTS, most of which correspond to the general formula
Cl(CH2 )2 .NR.(CH2 )2 Cl. They are toxic (e.g. causing blisters on
contact with the skin), mutagenic and carcinogenic, and promote
IMMUNOSUPPRESSION. Nitrogen mustards (and the SULPHUR
MUSTARDS) react with DNA e.g. at the N-7 position of guanine
residues, forming mono-adducts as well as inter- and intra-strand
cross-links.
nitrogen-regulated genes See NTR GENES.
nitrogenase (dinitrogenase) An enzyme complex (EC 1.18.2.1)
which catalyses biological NITROGEN FIXATION: it combines with
N2 and reduces it to NH3 . Nitrogenase can also reduce other
substrates e.g., acetylene, azide, cyanide, nitrous oxide; the
reduction of acetylene to ethylene (detectable by gas chromatography) is the basis of an assay for nitrogenase. The nitrogenase
complex typically comprises two components: the MoFe (or
FeMo) protein (also called e.g. component I, molybdoferredoxin,
azofermo, or dinitrogenase), and the Fe protein (= e.g. component II, azoferredoxin, azofer, dinitrogenase reductase). The
MoFe protein (MWt ca. 220000250000) is an a2 b2 tetramer
containing ca. 50 iron atoms, 2 molybdenum atoms, and ca. 30
acid-labile sulphide groups; the molybdenum occurs in an FeMo
cofactor (FeMoco) containing at least 1Mo per 6Fe [ARB (1984)
53 231257]. (An alternative nitrogenase has been found in a
strain of Azotobacter chroococcum in which the MoFe protein is
replaced by a vanadium-containing protein [Nature (1986) 322
388390].) The Fe protein (MWt ca. 5500060000) contains
two identical protein subunits, 4 iron atoms and 4 acid-labile
sulphide groups. The substrate (e.g. N2 ) is bound by the MoFe
protein and, in the presence of Mg-ATP, electrons are transferred
from reduced ferredoxin or flavodoxin to the Fe protein which, in
turn, reduces the MoFe protein with concomitant ATP hydrolysis. (At least 2ATP are hydrolysed for each electron transferred.)
In an apparently inevitable side-reaction of nitrogenase, electrons are transferred to protons, resulting in the ATP-dependent
evolution of H2 ; H2 evolution thus competes with nitrogen fixation for energy and reducing power. Some organisms (e.g. some
Rhizobium bacteroids [Book ref. 55, pp. 179203], Azotobacter spp, and some cyanobacteria) possess an oxygen-dependent
enzyme system termed uptake hydrogenase which oxidizes the
H2 to yield ATP; this enzyme system also serves to remove H2
NODULES
CHODESMIUM.)
523
Nitrosospira
cytotoxic T cells which are MHC class I-restricted. (NK cells
are not MHC class I-restricted; in fact, class I molecules inhibit
the killing activity of NK cells.) This role of NK cells appears to
be particularly valuable in that many viruses are able to inhibit
the display of MHC class I-linked viral antigens at the cell
surface.
The killing activity of NK cells is stimulated by certain
cytokines, including INTERLEUKIN 12.
NLF A non-lactose-fermenting bacterium.
nm (nanometre) 109 m, or 103 m.
NMR NUCLEAR MAGNETIC RESONANCE.
NNN medium (Novy, Nicolle and MacNeals medium) A DIPHASIC MEDIUM used e.g. for the culture of certain Leishmania spp
and stercorarian trypanosomes. It is a blood agar SLOPE (containing defibrinated mammalian blood) to which has been added a
small volume of e.g. Lockes solution containing antibiotics to
inhibit bacterial growth. The inoculated slope is incubated (e.g.
2528 C) for days or weeks; a loopful of fluid can be removed
at intervals for examination.
In culture, pathogenic flagellates may form only certain morphological types; Leishmania donovani grows in the promastigote form, although Trypanosoma cruzi cultures contain e.g. epimastigotes and metacyclic forms.
NNRTI NON-NUCLEOSIDE REVERSE TRANSCRIPTASE INHIBITOR.
Noble agar A purified (washed) form of AGAR.
noble rot (pourriture noble; Edelfaule) A rot of grapes caused
by Botrytis cinerea. On ripe or over-ripe white grapes the mould
penetrates the grape skins and leads to loss of water; must from
such grapes is thus more concentrated than normal and is used
for making high-quality sweet wines (see WINE-MAKING). (The
same mould on unripe or black grapes renders them useless for
wine-making.)
nocardamine A colourless, trihydroxamate SIDEROPHORE produced e.g. by certain actinomycetes and by Pseudomonas stutzeri
under iron-deficient conditions. [JGM (1980) 118 125129.]
Nocardia
A genus of Gram-positive, aerobic, chemoorganotrophic, non-motile bacteria (order ACTINOMYCETALES, wall type
IV) which occur e.g. in soil and as pathogens of man and
other animals (see e.g. MADUROMYCOSIS, NOCARDIOSIS; see also
NOCARDICINS); the degree of acid-fastness appears to be variable even within a given isolate. The organisms typically form a
branched (substrate and aerial) mycelium (hyphae 1 m or less
in diam.) which, according to species, tends to fragment more
or less readily into rods and coccoid forms, some of the latter
being heat- and/or desiccation-resistant (see MICROCYST (1)). Cell
walls contain MYCOLIC ACIDS. Growth occurs readily at 30 C and
37 C on enriched media; colonies are often wrinkled or ridged,
and may be any of a variety of colours. Glucose is metabolized
oxidatively. GC%: 6472. Type species: N. asteroides.
The genus includes e.g. N. amarae (isolated e.g. from the
foam on an activated-sludge sewage treatment plant) and
also N. asteroides, N. brasiliensis and N. farcinica (Kyoto-1
group), N. otitidis-caviarum, and N. vaccinii (a species reported
to produce galls in the blueberry plant). N. autotrophica,
N. mediterranea and N. rugosa each have type IV
actinomycete walls but they do not contain mycolic acids and
have been removed from the genus [Book ref. 73, pp. 8991,
129].
(See also e.g. HYDROCARBONS and RUBBER SPOILAGE.)
nocardicins A class of monocyclic b-LACTAM ANTIBIOTICS (q.v.
for structure) produced by a species of Nocardia.
nocardioform actinomycetes A category within the order ACTINOMYCETALES which includes Caseobacter, Corynebacterium,
non-motile or motile with 12 subpolar flagella. The cells contain lamellar cytomembranes in a mainly peripheral arrangement.
Marine strains (and some other strains) have an S LAYER. (See
also CARBOXYSOMES.) GC%: ca. 4751.
Nitrosospira A genus of Gram-negative bacteria of the NITROBACTERACEAE; the organisms occur in soil. Under the light microscope the cells appear as rods, ca. 0.30.4 0.81.0 m, but
they appear as tightly coiled spirals under the electron microscope; the cells may be non-motile, or motile with 16 flagella,
and they divide by binary fission. Cytomembranes are absent.
Type species: N. briensis. GC%: ca. 54.
nitrosoureas See N-NITROSO COMPOUNDS.
Nitrosovibrio
A genus of Gram-negative bacteria of the
NITROBACTERACEAE. The type species, N. tenuis, is represented
by a single isolate from soil in the Hawaiian Islands; cells:
straight to curved rods, ca. 0.30.4 1.13.0 m (coccoid in
stationary-phase cultures), with 14 lateral or subpolar flagella.
Extensive cytomembranes are lacking. Cells divide by binary
fission.
Nitrospina A genus of Gram-negative marine bacteria of the
NITROBACTERACEAE. Cells of the type species, N. gracilis, are
non-motile rods, ca. 0.30.4 2.66.5 m, which divide by
binary fission; the cells may contain numerous deposits of
glycogen. GC%: ca. 58. (See also CARBOXYSOMES.)
nitrous acid (as a MUTAGEN) Nitrous acid (HNO2 ) can cause the
oxidative deamination of guanine (G), cytosine (C) and adenine
(A) to form xanthine (X), uracil (U) and hypoxanthine (HX),
respectively. When DNA treated with nitrous acid undergoes
replication, X pairs with C which, on subsequent replication,
pairs with G: i.e., no mutation results from G deamination. U
pairs with A, and HX pairs with C: thus deamination of C and
A leads to GC-to-AT and AT-to-GC transitions, respectively.
(HNO2 can also cause e.g. cross-linking between bases.)
In e.g. Escherichia coli the abnormal bases HX and U can be
removed from DNA by specific hypoxanthine- and URACIL-DNA
GLYCOSYLASES.
Nitschkea See SORDARIALES.
Nitzschia See DIATOMS.
nivalenol See TRICHOTHECENES.
NK cells Natural killer cells: lymphoid cells, derived from bone
marrow stem cells, which are related to, but antigenically distinct
from, T LYMPHOCYTES; NK cells do not express the T cell receptor
(TCR), and do not express CD3, CD4 or CD8 antigens but they
do express the CD16 antigen. NK cells are classified as large
granular lymphocytes (LGLs).
NK cells have little phagocytic activity, but they can exert
cytotoxic/cytolytic activity against various pathogens, against
host cells infected with certain bacteria (e.g. Listeria monocytogenes) or viruses, and against certain tumours; moreover, NK
cells can be stimulated to release CYTOKINES, including IFN-g
(see INTERFERONS).
NK cells may bind to target cells (e.g. virus-infected cells)
via the CD16 receptor i.e. CD16 binding to the Fc portion
of antibodies that have bound to the target cell (see ADCC).
Alternatively, binding to target cells may occur in an antibodyindependent way receptors on NK cells binding directly to
ligands on the target cell.
The killing activity of NK cells appears to involve the release
of perforins and granzymes which induce APOPTOSIS in target
cells.
NK cells can attack virus-infected host cells which do not
express viral antigen, linked to MHC class I molecules, at the
cell surface; such cells would not normally be targeted by CD8+
524
nomenclature
Mycobacterium, Nocardia and Rhodococcus organisms which
form either non-mycelial growth or a fragmenting mycelium
and which have a cell wall of chemotype IV. (cf. SPOROACTINOMYCETES.)
Nocardioides A genus of aerobic soil bacteria (order ACTINOMYCETALES, wall type I) which form branching substrate and aerial
mycelia that fragment into coccoid and rod-shaped pieces. GC%:
ca. 6667. Type species: N. albus. [Book ref. 73, pp. 100101.]
Nocardiopsis A genus of bacteria (order ACTINOMYCETALES, wall
type III) which occur e.g. in soil. The organisms form branching,
fragmenting substrate mycelium, and an aerial mycelium which
gives rise to long chains of spores each spore tending to
form at an angle to its neighbours, thus giving the chain
an undulating appearance. GC%: ca. 7076. Type species:
N. dassonvillei (formerly Actinomadura dassonvillei ). [Book
ref. 73, pp. 117118.]
nocardiosis An acute or chronic disease of man and animals,
caused by a species of Nocardia (commonly N. asteriodes). The
disease may be systemic: suppurative lesions are formed mainly
in the lungs, but the infection may disseminate to other organs
(brain, kidney etc). Nodular, often suppurating, subcutaneous
lesions may result from disseminated infection or from primary
infection via a wound. (See also MADUROMYCOSIS.)
nocardomycolic acids MYCOLIC ACIDS of Nocardia spp.
Noctiluca
A genus of marine, bioluminescent, heterotrophic
(holozoic) DINOFLAGELLATES. The vegetative cells are large (e.g.
2002000 m diam.), roughly spherical (with no girdle), and
have highly vacuolated cytoplasm; the flagella are very short,
the transverse flagellum being reduced to a small projection.
There is a deep sulcus from the region of which arises a
retractable tentacle; the tentacle is apparently sticky and aids
in the capture of prey. A cytostome is present near the base of
the tentacle. Some strains of Noctiluca contain endosymbiotic
unicellular green flagellates in vacuoles within the cell. (See also
BIOLUMINESCENCE.)
Nodamura virus See NODAVIRIDAE.
Nodaviridae (Nodamura virus group) A family of ssRNA viruses
which infect insects of the Diptera, Coleoptera and Lepidoptera.
The virions are roughly spherical, naked, 29 nm diam., and
each contains one major polypeptide species and two molecules
of non-polyadenylated ssRNA (MWts ca. 1.15 and 0.46
106 ), both of which are necessary for infection. The type
species, Nodamura virus, was isolated from mosquitoes (Culex
tritaeniorhynchus) in Japan; it can replicate in various insects,
can cause a lethal infection in suckling mice, and can replicate in
various vertebrate and invertebrate cell cultures (including e.g.
BHK cells). Other member: Black beetle virus, isolated from
the New Zealand Black beetle, Heteronychus arator. Possible
members include e.g. Arkansas bee virus.
Nodosaria See FORAMINIFERIDA.
Nodularia
A genus of filamentous freshwater and marine
(littoral) CYANOBACTERIA (section IV) in which the trichomes
are made up of disc-shaped vegetative cells. Heterocysts may
be intercalary or terminal. GC%: ca. 41. N. spumigena is a gasvacuolate, primarily freshwater, bloom-forming species which
may form toxin(s) responsible for severe vomiting and bloody
diarrhoea, or chronic liver and kidney damage, in animals which
drink the water.
nodules (plant microbiol.) See ACTINORRHIZAE; PHYLLOBACTERIUM; ROOT NODULES; STEM NODULES.
nodulins ROOT NODULE-specific proteins specified by host plant
genes; they appear to be involved in symbiotic nitrogen fixation and nitrogen metabolism. C-nodulins (common nodulins)
nomenspecies
NOMENCLATURE: some suffixes used in microbial nomenclature
Algae
Division (phylum)
Subdivision (subphylum)
Superclass
Class
Subclass
Superorder
Order
Suborder
Superfamily
Family
Subfamily
Tribe
Subtribe
Genus
Bacteria
Fungi
Protozoa
-phyta
-phytina
-mycota
-mycotina
-phyceae
-phycidae
-mycetes
-mycetidae
-a
-a
-a
-ea
-ia
-idea
-ida
-ina
-oidea
-idae
-inae
-ini
-ales
-ineae
-ales
-ineae
-ales
-ineae
-aceae
-oideae
-eae
-inae
-aceae
-oideae
-eae
-inae
-aceae
-oideae
-eae
-inae
Viruses
-viridae
-virinae
-virus
and B). It occur in large numbers (e.g. 106 copies per nucleus)
and binds to dsDNA in an apparently non-sequence-specific
manner although it binds strongly to specific DNA structures
such as angular or kinked DNA or four-way junctions. HMG1
can also interact with certain other DNA-binding proteins and,
in this way, can cause sharp bends to develop in dsDNA; this
ability can enhance the activity of certain transcription factors,
and HMG1 apparently affects the expression of particular genes.
HMG1 also has extra-nuclear activity. In vitro, it can be
secreted by macrophages on stimulation by CYTOKINES or ENDOTOXIN, and it may have a role e.g. in inflammation. More recently
it has been reported that HMG1 is released by certain damaged
or necrotic cells, including endothelial cells, and that it can act
as a chemoattractant, induce cell migration and bring about reorganization in the cytoskeleton in certain cells [JCB (2001) 152
11971206].
Nonidet P-40 A non-ionic detergent of the polyoxyethylene p-toctyl phenol series.
Nonion See FORAMINIFERIDA.
non-Mendelian inheritance Syn. CYTOPLASMIC INHERITANCE.
non-nucleoside reverse transcriptase inhibitors (NNRTIs) A
category of ANTIRETROVIRAL AGENTS (q.v.) that includes delavirdine, efavirenz and nevirapine. The NNRTIs are structurally
diverse compounds; they bind to reverse transcriptase and inhibit
enzyme activity. The clinically used NNRTIs are reported to
be effective against the reverse transcriptase of HIV-1 but not
against that of HIV-2. (See also NU-1320.)
[NNRTIs and other antiretroviral agents in the treatment of
AIDS: BMJ (2001) 322 14101412.]
non-O1 Vibrio cholerae pilus See NCVP.
non-permissive conditions See CONDITIONAL LETHAL MUTANT.
non-persistent transmission See NON-CIRCULATIVE TRANSMISSION.
non-photochromogen A term used (very loosely) to refer e.g.
to any strain of Mycobacterium which (i) forms little or no
pigment, (ii) does not form pigment during early growth, and/or
(iii) does not need to grow in the light in order to produce
pigment (cf. SCOTOCHROMOGEN).
non-propagative viruses See CIRCULATIVE TRANSMISSION.
non-reciprocal recombination See RECOMBINATION.
nonsense codon See GENETIC CODE.
nonsense mutation A MUTATION in which a codon specifying an
amino acid is altered to a nonsense (chain-terminating) codon:
e.g. an amber codon (amber mutation) or an ochre codon (ochre
mutation). (cf. MIS-SENSE MUTATION.)
nonsense suppressor See SUPPRESSOR MUTATION.
non-specific immunity The constitutive (or, in certain cases,
acquired) resistance of the body to foreign materials in general including those (living and non-living) materials with
which it has had no previous contact. Non-specific immunity
involves e.g. PHAGOCYTOSIS and the activities of INTERFERONS,
LYSOZYME and PROPERDIN. (cf. SPECIFIC IMMUNITY.)
non-specific immunization The administration of certain immunostimulants (e.g. BCG) in order to elicit a heightened immune
response to antigen(s) unrelated to the immunostimulant.
non-specific immunotherapy The therapeutic use of NONSPECIFIC IMMUNIZATION.
non-specific urethritis Syn. NON-GONOCOCCAL URETHRITIS.
non-specific vaginitis Syn. BACTERIAL VAGINOSIS.
non-sterilizing immunity Syn. PREMUNITION.
non-steroidal anti-inflammatory drugs (NSAIDs) See PROSTAGLANDINS.
non-sulphur purple bacteria See RHODOSPIRILLACEAE.
527
non-treponemal tests
in discrete cephalodia (see CEPHALODIUM). In liverworts (e.g.
Blasia, Cavicularia) and hornworts (Anthoceros), Nostoc occurs
in cavities in the underside of the thallus. Among angiosperms,
Gunnera (a genus of rhubarb-like marsh plants) contains Nostoc
punctiforme in mucilage-filled glands in the plant stem at
the bases of petioles; the cyanobiont penetrates between the
cortical cells and enters meristematic cells, thus becoming an
intracellular symbiont. [Development of Nostoc in Gunnera
mucilage glands: Bot. Gaz. (1985) 146 5662.] Cycads are the
only gymnosperms known to be capable via symbionts of
nitrogen fixation; they develop coralloid root nodules which
contain symbiotic nitrogen-fixing cyanobacteria (Nostoc) in
mucilage-filled spaces in the root cortex [ultrastructural studies
of NostocZamia association: New Phyt. (1985) 101 707716].
Nostocales See CYANOBACTERIA.
notatin A flavoprotein GLUCOSE OXIDASE produced intracellularly
e.g. by Penicillium notatum (= P. chrysogenum). It can show
antimicrobial activity due to the production of HYDROGEN
PEROXIDE.
NotI See RESTRICTION ENDONUCLEASE (table).
notifiable diseases Those diseases (of man, animals or plants) the
occurrence (or suspected occurrence) of which must, by law, be
notified to the appropriate authorities.
novel antigen Any weakly immunogenic or non-immunogenic
molecule which can be made (more) immunogenic by CONJUGATION (sense 2) with an immunogenic molecule. (cf. HAPTEN;
NEOANTIGEN.)
novobiocin (albamycin) An ANTIBIOTIC (produced e.g. by Streptomyces spheroides and S. niveus): 4,7-dihydroxy-3-amino-8methylcoumarin linked via the 3-amino group to a substituted
p-hydroxybenzoic acid and via the 7-hydroxy group to a substituted hexose (noviose). Novobiocin is more active against
Gram-positive than Gram-negative bacteria; resistance develops
readily. It primarily inhibits synthesis of DNA and, to a lesser
extent, RNA. It selectively and competitively inhibits the binding of ATP to GYRASE B subunits; thus DNA supercoiling by
gyrase is inhibited, but the (ATP-independent) DNA-relaxing
gyrase activity is not. (See also CURING.) Secondary effects of
novobiocin include inhibition of protein and cell wall synthesis.
(See also COUMERMYCINS; cf. NALIDIXIC ACID.)
Novyella A subgenus of PLASMODIUM.
Nowakowskiella A genus of eucarpic, polycentric fungi (order
CHYTRIDIALES) which are typically aquatic saprotrophs. The
vegetative thallus includes a RHIZOMYCELIUM whose branching
rhizoids penetrate the substratum. Operculate zoosporangia are
formed, and each liberated zoospore germinates to form a
rhizomycelium. Thick-walled resting spores are formed on
pseudoparenchymatous structures, but whether or not these are
sexual structures is unknown.
noxythiolin (N-methyl-N -hydroxymethylthiourea) A broadspectrum antimicrobial agent which has been used e.g. for
the treatment of bacterial peritonitis; its activity appears to
depend on the release of FORMALDEHYDE. Noxythiolin can kill
blastospores of Candida albicans in vitro [JAB (1986) 60
319325].
nPCR See NESTED PCR.
NPV NUCLEAR POLYHEDROSIS VIRUS.
NR1 plasmid See R100 PLASMID.
nrdA gene (dnaF gene) A gene which codes for ribonucleotide
reductase.
nrdB gene See SPLIT GENE (e).
nrdD gene See SPLIT GENE (e).
NifL
NifA
nifLA
54
ntrC
ntrB
54
54
rpoN
ntr GENES: control of the nif genes by the ntr genes in Klebsiella pneumoniae (diagrammatic) (see entry). Transcription of all the nif
genes/operons requires the enhancer-dependent sigma factor s54 (rpoN gene product); additionally, transcription initially requires an activated
(phosphorylated) NtrC protein which is present when combined nitrogen is limiting. NtrB is apparently involved in regulating the activity of
NtrC.
The first nif genes to be transcribed are those in the nifLA operon. NifA, which is functionally related to NtrC, takes over the role of activator
of E s54 for all subsequent nif genes/operons. NifL can inhibit NifA in the presence of combined nitrogen; moreover, NifA is inactivated by
oxygen. Nitrogen fixation is blocked completely by null mutations in rpoN, ntrC or nifA.
529
nuclear petite
can be detected by its ability to induce a signal (a radiofrequency
alternating voltage) in a coil tuned to the particular resonance
frequency. Usually, a single excitatory pulse produces only
a weak resonance signal, so that several hundred or several
thousand intermittent pulses are commonly used, the resulting
resonance signals being added together in a computer.
The resonance frequency of a given nucleus is influenced
by the precise location of the atom within a molecule: if
atoms of a given type (e.g. 1 H) are located in different
molecular environments (e.g. CH2 , CH3 , OH) their nuclei will
have slightly different resonance frequencies. When, due to
a chemical reaction, an atom moves to a different molecular
environment, the resonance frequency of its nucleus will change
to that specified by the new location. A given type of nucleus
within a particular molecular environment may be identified
by its chemical shift (d): the relative amount by which its
resonance frequency is shifted from that of a given reference
standard which, for 1 H, is the agent tetramethylsilane (TMS),
(CH3 )4 Si; chemical shift is expressed in the dimensionless unit
parts per million (ppm).
If, for a given type of nucleus (e.g. 1 H), the nuclear resonance
frequency is determined (under standard conditions) for each
type of molecular environment, it is possible e.g. to follow the
progress of a chemical reaction by monitoring changes in signal
strength at the various resonance frequencies; this is possible
because the signal strength at a given resonance frequency is
proportional to the number of nuclei occupying a given type of
molecular environment.
An NMR signal is a composite radio-frequency trace which
incorporates simultaneous signals at various resonance frequencies; it is called a free induction decay (FID) since signal intensity decreases to zero as all the nuclei relax into their former
(pre-excited) state of thermal equilibrium. The various resonance
signals are separated out from the FID by mathematical manipulation involving the Fourier transform: a function which relates
a complex waveform to its component spectrum of frequencies.
The apparatus used for NMR includes an electromagnet or
a superconducting magnet in order to obtain a strong magnetic
field. Field strength directly influences the absolute resonance
frequencies of nuclei; thus, e.g., resonance frequencies of 1 H
nuclei are centred around ca. 42.6 megacycles (= megahertz,
MHz) when the magnetic field is 1 tesla (= 10000 gauss), while
at 4.7 tesla the 1 H nucleus resonates at ca. 200 MHz. Other
resonance frequencies include e.g. (MHz per tesla): 10.7(13 C),
4.31(15 N) and 17.24 (31 P).
[Book ref. 151; NMR and its clinical applications: BMB
(1984) 40 113201; NMR in biochemistry: Book ref. 152,
pp. 167; NMR and drug design: Book ref. 153, pp. 267281;
microbiological applications of NMR: MS (1985) 2 203211,
340345.]
nuclear petite See PETITE MUTANT.
nuclear polyhedrosis viruses (NPVs) Viruses belonging to subgroup A of the BACULOVIRIDAE (q.v.). Virus replication and occlusion body formation occur exclusively in the host cell nucleus
(cf. CYTOPLASMIC POLYHEDROSIS VIRUS GROUP). The NPV virion
may contain a single nucleocapsid (S NPV) or many nucleocapsids (M NPV). Type species: Autographa californica NPV
(AcM NPV); other members include e.g. Bombyx mori (silkworm) NPV (BmS NPV), Orygia pseudotsugata (Douglas Fir
tussock moth) NPVs (OpS NPV and OpM NPV), and viruses
from many other insects and from certain crustacea.
Nuclearia A genus of amoebae (class FILOSEA). N. delicatula
feeds by ingesting filamentous cyanobacteria [feeding behaviour
and structure: JP (1986) 33 369374].
C
6
N1
HN 1
7
8
HC 2
4C
H2N
CH
5
6
CH
N
7
C2
CH
N
H
N
guanine
NH2
4
N
H
adenine
N3
CH
HN 3
O
C2
O
C
5
6
C
CH
CH3
HN 3
O
C2
5 CH
6
N
H
N
H
N
H
cytosine
thymine
uracil
CH
NUCLEOSIDE: some of the bases commonly found in nucleosides. Reproduced from Bacteria 5th edition, Figure 7.3, page 112, Paul Singleton
(1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4) with permission from the publisher.
Base
OH
5
HO
CH2 O
O
H
H
3
OH OH
531
null cells
formed at the 100% level of similarity. Although strains within
a given cluster are mutually 100% similar, no information is
given here on the degree of similarity which exists between the
OTUs of one cluster and those of another. The remaining OTUs
are progressively added at successive, lower levels of similarity
(e.g. 97%, 95%, 80%, 75%, 50%) to one or other of the initially
formed clusters. Additionally, two or more clusters may unite at
a given level of similarity; thus, e.g. in the above example the
clusters 4347 and 293133 may form a single cluster at,
say, 75% meaning that one or more OTUs in a given cluster
has a mutual similarity of at least 75% with one or more OTUs
in the other cluster. The mode in which OTUs are added to a
cluster, and in which clusters unite, may be varied according
to the purpose of the taxonomist: see e.g. SINGLE LINKAGE and
UPGMA. At the end of the study the result of clustering may
be shown e.g. in a PHENOGRAM or in a SHADED MATRIX. The
processed data can then be examined to determine whether or
not a given phenon can be regarded as a TAXON.
Nummilites See FORAMINIFERIDA.
nummilitids See FORAMINIFERIDA.
nungham The freshwater red alga Lemanea mamillosa (division
RHODOPHYTA) used as a food in India.
nu/nu mice A strain of congenitally athymic mice.
nusA gene See TRANSCRIPTION and BACTERIOPHAGE LAMBDA.
nutrient agar NUTRIENT BROTH gelled with 1.52.0% AGAR: a
general-purpose solid basal MEDIUM.
nutrient broth A liquid basal MEDIUM; the name may refer to
either extract broth or infusion broth. Extract broth (the type
most commonly used) may be prepared as an aqueous solution
of beef extract and peptone (each ca. 0.51.0% w/v) and sodium
chloride (ca. 0.5% w/v); it is sterilized by autoclaving, and the
final pH is ca. 7.27.4. Powdered (dehydrated) extract broth
is available commercially; it is reconstituted with distilled (or
tap) water, dispensed into tubes, and autoclaved. Infusion broth
is prepared by infusing overnight, at 4 C, 50 g of minced lean
beef in 100 ml distilled water; peptone (ca. 1% w/v) and sodium
chloride (ca. 0.5% w/v) are added, and the mixture is boiled,
filtered, and sterilized by autoclaving. Final pH: ca. 7.37.5.
nutritionally variant streptococci (NVS) Strains of Streptococcus, present e.g. in the normal human throat and urogenital
tract, which are characterized by a requirement for cysteine,
or for pyridoxal hydrochloride or pyridoxamine hydrochloride,
when grown on complex media; the organisms were originally
detected as satellite colonies (see SATELLITE PHENOMENON) of viridans streptococci associated with colonies of Staphylococcus.
Two species are distinguished: S. adjacens and S. defectivus, the
latter species differing from S. adjacens e.g. in fermenting trehalose and forming b-galactosidase. The organisms may form a
red pigment. NVS may be responsible for 5% of those cases
of endocarditis which involve oral streptococci.
Nuttallia See BABESIA.
nvCJD New variant CREUTZFELDTJAKOB DISEASE.
NVDP See PLASMODIUM.
NVL No visible lesion.
NVS NUTRITIONALLY VARIANT STREPTOCOCCI.
Nycodenz See IODINATED DENSITY-GRADIENT MEDIA.
nystatin (fungicidin) An antifungal POLYENE ANTIBIOTIC, produced
by Streptomyces noursei and named after the New York State
Health Department (where it was discovered). It contains
MYCOSAMINE and is usually classed as a tetraene, although it
contains six double bonds (four conjugated double bonds separated
from two others by two methylene groups). Nystatin is used
primarily for the topical treatment of superficial mycoses (e.g.
mucosal Candida infections); it is not absorbed when taken orally.
5101119
4347
293133
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
O
O antigens (Boivin antigens) The heat-stable, alcohol-resistant
LIPOPOLYSACCHARIDE protein somatic antigens of Gram-negative
bacteria (particularly members of the Enterobacteriaceae); O
antigens are important in the serological characterization of enterobacteria (see e.g. KAUFFMANNWHITE CLASSIFICATION). Antigenic
specificity is determined by the polysaccharide O-specific chains
(see LIPOPOLYSACCHARIDE). O antigens may be modified e.g. by
BACTERIOPHAGE CONVERSION or by mutation (e.g. in salmonellae
a mutation may give rise to T1 side-chains, consisting of ribose
and galactose residues, instead of normal O-specific chains see
also SMOOTHROUGH VARIATION). (See also VI ANTIGENS.)
O side chain See LIPOPOLYSACCHARIDE.
O-specific chain See LIPOPOLYSACCHARIDE.
O-type starter See LACTIC ACID STARTERS.
O1 strains (of Vibrio cholerae) See VIBRIO.
O/129 2,4-Diamino-6,7-diisopropylpteridine: a water-soluble
agent bacteriostatic for e.g. many members of the Vibrionaceae
(e.g. most Vibrio strains). Sensitivity to O/129 may be determined using O/129-impregnated discs on nutrient agar containing 0.5% w/v NaCl.
Some strains of Vibrio cholerae produce a trimethoprimresistant dihydrofolate reductase (DHFR) and are resistant to
both trimethoprim and O/129; the gene encoding the DHFR may
be borne on a plasmid or on a transposon [Ann. Mic. (1985)
136B 265273].
O139 Bengal (Vibrio cholerae) See CHOLERA.
O157:H7 E. coli See EHEC.
oak butt rot See BUTT ROT.
oak-moss Evernia prunastri.
oak wilt A disease of oak trees (Quercus spp) caused by
Ceratocystis fagacearum. Infection occurs via wounds (made
e.g. by man or woodpeckers). The fungus forms pressure
cushions (sclerotia) between the infected xylem and phloem,
bursting open the overlying bark and allowing entry of insects,
particularly sap-feeding beetles of the Nitidulidae, which act as
vectors of the disease.
OakleyFulthorpe test See DOUBLE DIFFUSION.
oar weed Any species of Laminaria which has an oar-shaped
thallus, e.g. L. digitata and L. hyperborea.
oat diseases See CEREAL DISEASES.
oat mosaic virus See POTYVIRUSES.
oat necrotic mottle virus See POTYVIRUSES.
oat sterile dwarf virus See FIJIVIRUS.
oat striate virus See RHABDOVIRIDAE.
Obesumbacterium A genus of non-motile, slow-growing bacteria of the ENTEROBACTERIACEAE (apparently related to Hafnia
alvei ), found as contaminants in fermenting beer wort. Cells:
pleomorphic rods, 0.82.0 1.5100 m (short, fat rods predominate in wort). [Book ref. 22, pp. 506509.]
objective (objective lens) See MICROSCOPY (a).
obligate Refers to an essential attribute of a given organism. For
example, an obligate aerobe is an organism which grows only
under aerobic conditions, and an obligate parasite is an organism
which, in nature, can grow only as a parasite. (cf. FACULTATIVE.)
obligate proton reducers See ANAEROBIC DIGESTION.
Obodhiang virus See LYSSAVIRUS.
occlusion bodies See BACULOVIRIDAE.
Occlusosporida See STELLATOSPOREA.
oncogene
Members of the suborder Oligotrichina are typically small
and rounded organisms whose somatic ciliature may consist of
only a few short rows of bristles, but which may have groups
of cirri or bristles forming an equatorially encircling band;
genera include e.g. HALTERIA, Strombidium, Strombilidium, and
Tontonia.
The other suborder, TINTINNINA (q.v.), comprises a distinctive
group of organisms.
Oligotrichina See OLIGOTRICHIDA.
oligotroph Any organism which can grow in relatively nutrientpoor environments (cf. COPIOTROPH).
oligotrophic (1) Of or pertaining to an OLIGOTROPH. (2) Of lakes,
rivers etc: containing low levels of nutrients, particularly of those
nutrients which support the growth of aerobic photosynthetic
organisms. (cf. EUTROPHIC.)
olivanic acids An ill-defined group of CARBAPENEM antibiotics derived from Streptomyces olivaceus and other Streptomyces spp.
olive-green mould Chaetomium olivaceum: a mould which frequently grows on mushroom compost after pasteurization (see
MUSHROOM CULTIVATION) and which inhibits mycelial development in Agaricus brunnescens by competition for nutrients.
[Biological control by a thermophilic Bacillus sp: AEM (1983)
45 511515.]
olive knot A disease of the olive, oleander and privet, in which
small galls develop on young twigs and leaves. The causal agent
is Pseudomonas syringae pv. savastanoi ; the pathogen produces
IAA and cytokinin which may be responsible for the formation
of the galls. In at least some strains IAA production appears to
be plasmid-mediated. Infection occurs via wounds. Transmission
may occur via the olive fly (Dacus oleae).
olives (pickled) See PICKLING.
olivomycin See CHROMOMYCIN.
Olpidiopsis See LAGENIDIALES.
Olpidium A genus of unicellular, endobiotic, holocarpic fungi
(order CHYTRIDIALES) which are parasitic on algae and other
aquatic organisms and on some terrestrial plants; Olpidium
spp are also involved in the transmission of the LETTUCE BIG
VEIN AGENT and the TOBACCO NECROSIS VIRUS. In the asexual
cycle of O. viciae a zoospore settles on a susceptible host
(Vicia), encysts, and the cysts contents enter a host cell; after
intracellular growth and a number of nuclear divisions, the
fungus eventually forms an inoperculate zoosporangium the
numerous zoospores subsequently escaping via one or more
pores. In the sexual cycle, two morphologically indistinguishable
zoospores fuse and then encyst on a susceptible host; the cysts
contents enter a host cell and develop into thick-walled resting
sporangia. Karyogamy (and probably meiosis) occur before the
germination of resting sporangia each of which produces a
number of zoospores.
OM OUTER MEMBRANE.
omasum See RUMEN.
OMearas method See VOGESPROSKAUER TEST.
!-oxidation See HYDROCARBONS.
! (omega) protein See TOPOISOMERASE.
omicron An endosymbiotic, Gram-negative, rod-shaped bacterium which occurs in the cytoplasm of Euplotes spp; it does
not confer a killer characteristic, and it appears to be essential
for the viability of its protozoan host. [Book ref. 22, p. 798.]
omnivorous Refers to protozoa which feed on microscopic
animals (e.g. other protozoa) and plants (e.g. algae, bacteria).
(cf. CARNIVOROUS; HERBIVOROUS.)
Omp The designation of certain major OUTER MEMBRANE PROTEINS, each type of protein being distinguished as OmpA, OmpC
etc. Some of these proteins are PORINS for example OmpC and
OmpF (see OSMOREGULATION). In Escherichia coli, OmpA (also
called e.g. 3A, d and II ) is a product of the ompA gene (also
called e.g. con, tolG and tut); it apparently spans the thickness
of the outer membrane but does not seem to function as a porin.
OmpA-deficient mutants have an unstable outer membrane and
are deficient in conjugation and in sensitivity to colicin L and
phages K3 and TuII. In E. coli, OmpT is a protease involved in
type IV (autotransporter) protein secretion.
OMP Orotidine 5 -monophosphate [see Appendix V(b)].
OmpA See OMP.
Omphalotus See AGARICALES (Tricholomataceae).
OmpR See OSMOREGULATION.
OmpT protein See PROTEIN SECRETION (type IV systems).
Omsk haemorrhagic fever See VIRAL HAEMORRHAGIC FEVERS
and FLAVIVIRIDAE.
onc See ONCOGENE.
Oncobasidium See TULASNELLALES and VASCULAR-STREAK DIEBACK.
oncogen See ONCOGENIC.
oncogene A gene which can (potentially) induce neoplastic transformation in the cell in which it occurs or into which it is
introduced. Oncogenes occur e.g. in certain viruses, particularly members of the RETROVIRIDAE. Viral oncogenes (v-onc),
originally identified as the transforming determinants of acutely
oncogenic retroviruses, were subsequently found to have closely
related cellular homologues (designated c-onc or proto-onc) in
the chromosomes of eukaryotes; c-onc sequences have been
highly conserved through evolution, and homologous genes have
been found in all vertebrates examined, as well as in lower
eukaryotes such as Drosophila and Saccharomyces. In the normal cell, at least some oncogenes are known to have one or
more major roles in cell growth/development. Retroviral v-onc
sequences may have arisen from c-onc genes by recombination
(see RETROVIRIDAE) and may differ from them e.g. in lacking
introns; they are often expressed with adjacent viral sequences
as fusion proteins.
Retroviral and cellular oncogenes are usually referred to by
three-letter designations based on the retrovirus in which they
were first identified: e.g. myc from myelocytomatosis virus, fes
from feline sarcoma virus, etc; viral genes are prefixed by v- (e.g.
v-myc), their cellular homologues by c- or proto- (e.g. c-myc or
proto-myc).
A v-onc gene introduced into a cell by an infecting retrovirus
may induce the neoplastic transformation of that cell in various
ways. The products of many retroviral oncogenes (e.g. v-abl,
v-fes, v-fps, v-ros, v-src, v-yes) have tyrosine-specific protein
kinase activity, transferring g-phosphate from ATP (or GTP) to
tyrosine residues in proteins. (See ABL, FES and SRC; cf. ERB and
MOS.) In normal (non-neoplastic) cells, tyrosine kinase activity
is associated with the receptors for certain growth-promoting
peptides: e.g. epidermal growth factor (EGF), platelet-derived
growth factor (PDGF) and insulin. Oncogenic tyrosine kinase
activity has been targeted by selective inhibitors of proteins
encoded by e.g. bcr-abl and v-abl ; some inhibitors can be effective against a range of oncogenic kinases [e.g. Pharmacology
and Experimental Therapeutics (2000) 295 139145], and this
has encouraged the screening of existing clinically useful drugs
for activity against the emergent drug-resistant mutant kinases
[PNAS (2005) 102 1101111016].
v-myc and v-myb products lack tyrosine kinase activity (see
MYC and MYB). v-sis encodes a protein almost identical to the B
chain of human PDGF.
535
oncogenesis
of giving rise to a single plaque regardless of the number of
virions it may contain. (The latent period lasts ca. 2025 min
in phage T2/Escherichia coli B systems, but may be of the
order of hours in virus-infected animal cells.) Aliquots taken
sequentially after the latent period give progressively increasing
numbers of plaques; during this period the infected cells begin to
lyse, releasing large numbers of infectious virions each capable
of giving rise to a plaque. The number of plaques per aliquot
reaches a plateau when all the cells have lysed. (See also BURST
SIZE.) If the virions are labile the plateau is followed by a decay
period characterized by a fall in plaque titres.
If, during the latent period, the cells in each aliquot are lysed
artificially e.g. by the addition of SDS (for animal cells) or
chloroform (for Gram-negative bacteria) a so-called eclipse
period can be distinguished. In this period, which begins at the
same time as the latent period, infectious virions cannot usually
be detected owing to the uncoating of the virus following
infection; the eclipse period ends when the first progeny virions
are assembled. (The latent period normally continues until the
host cell lyses naturally, i.e., after the assembly of many progeny
virions.)
one-tube nPCR See NESTED PCR.
one-way incompatibility INCOMPATIBILITY exhibited by two given
plasmids only when one particular plasmid is introduced into a
cell containing the other; if the second plasmid is introduced
into a cell containing the first, incompatibility is not exhibited.
[One-way incompatibility between IncH1 plasmids and the F
plasmid: JGM (1985) 131 15231530.]
onion rot White rot (which can also affect e.g. leeks) is caused
by Sclerotium cepivorum; leaves become yellow and die, and the
rotting roots and scale bases become covered with white, fluffy
mycelium. Black sclerotia develop in or on necrotic tissue. Neck
rot, caused by Botrytis aclada (= B. allii), is more common in
stored onions. A soft rot can be caused by Burkholderia cepacia
(formerly Pseudomonas cepacia). (See also SMUDGE).
onion yellow dwarf virus See POTYVIRUSES.
onium compounds Syn. QUATERNARY AMMONIUM COMPOUNDS.
ONPG test A test used to detect b-D-galactosidase activity in bacteria. A loopful of growth of the test organism
(grown on e.g. TSI agar) is introduced into phosphate-buffered
peptone water (pH 7.0) containing ONPG (o-nitrophenyl-b-Dgalactopyranoside); the medium is then incubated at 37 C.
b-GALACTOSIDASE hydrolyses ONPG to galactose and o-nitrophenol the latter (being yellow) acting as a test indicator.
Organisms which give a positive ONPG test do not necessarily metabolize lactose since they may not synthesize a lactose
permease. (ONPG can enter cells without a specific permease.)
ontjom Syn. ONCOM.
ontogeny The range of stages which occur during the development of an individual organism to the mature or adult stage. The
supposition that ontogeny recapitulates PHYLOGENY (the law of
recapitulation or the recapitulation theory) was made by the
19th-Century biologist Haeckel.
onychomycosis MYCOSIS of nails (cf. PARONYCHIA). [Review:
Clinical Microbiology Reviews (1998) 11 415429.]
Onygena See GYMNOASCALES.
onyong-nyong fever (joint-breaker fever) A human disease
caused by an ALPHAVIRUS and transmitted by anopheline mosquitoes; it occurs e.g. in Africa. Symptoms: fever, headache,
myalgia, maculopapular rash, and severe arthralgia. Wild primates
may act as a reservoir of the virus.
oocyst (1) (mycol.) Syn. OOGONIUM. (2) (protozool.) A structure
in which sporozoites are formed. (3) An encysted fertilized
female gamete.
operator
[Role of Opa proteins in interactions with host (eukaryotic)
cells: TIM (1998) 6 489495.]
opacity-associated proteins (of Neisseria) See OPA PROTEINS.
opal codon See GENETIC CODE.
Opalina See OPALINATA.
Opalinata A subphylum of protozoa (phylum SARCOMASTIGOPHORA); the organisms are typically parasitic in amphibians.
Individual cells are often oval or elongated, ca. 60600 m in
length (according to species), and are generally flattened and
leaf-like; each contains two or more (typically many) identical
nuclei, and none has a cytostome. Each cell bears many short
flagella (which are described as cilia by some authors). Asexual
reproduction typically occurs by longitudinal (INTERKINETAL)
binary fission. In Opalina spp (rectal parasites of the frog) a
phase of rapid asexual multiplication and encystment coincides
with the breeding season of its amphibian host; it is believed
that this phase is triggered by the hosts hormonal activity.
Cysts, the infective stages, are voided by the frog and ingested
by tadpoles in which excystment is followed by repeated
longitudinal fission and the production of flagellated gametes.
After syngamy, the encysted zygote is voided and ingested by
another tadpole in which the zygote may undergo fission and
gamete formation, or develop to form the mature, multinucleate
trophic stage. (See also ENTAMOEBA (E. paulista).) Other genera
include Cepedea and Zelleriella.
Opegrapha A genus of crustose LICHENS (order OPEGRAPHALES).
Photobiont: Trentepohlia. Fruiting structures may be lirelliform
(see LIRELLA) or rounded. Species occur on rocks, bark etc.
Opegraphales An order of fungi of the ASCOMYCOTINA; members include crustose to fruticose LICHENS (photobiont commonly
trentepohlioid) and lichenicolous fungi. Ascocarp: APOTHECIOID,
with a typically thick, carbonaceous excipulum. Asci: bitunicate, elongated to clavate. Genera: e.g. Lecanactis, OPEGRAPHA,
ROCCELLA.
open complex See TRANSCRIPTION.
open culture Syn. CONTINUOUS CULTURE.
open reading frame (ORF) A sequence of codons (see GENETIC
CODE), starting with an initiator codon and ending with a
stop codon, which encodes a known or (as yet) unidentified
polypeptideor (see later) part of a polypeptide; the existence of
an ORF is revealed by sequencing studies (see DNA SEQUENCING).
A reading frame is said to be blocked if a stop codon is located
close to the initiator codon.
In some cases, two adjacent ORFs jointly encode a single
polypeptide; translation of such a polypeptide requires some
kind of mechanism (see e.g. READTHROUGH) that permits such
coupling. In one case, the mechanism of translational bypassing
of a 50-nucleotide gap between two ORFs appears to involve (i)
a stemloop structure between the first ORF and the coding
gap, and (ii) a sequence of amino acid residues within the
nascent peptide translated from the first ORF [EMBO (2000)
19 26712680].
open-system culture Syn. CONTINUOUS CULTURE.
operational taxonomic unit See OTU.
operator (mol. biol.) Any specific nucleotide sequence to which
a regulatory element can bind in order to control the expression
(transcription) of a given gene or operon. An operator commonly
consists of, or contains, a PALINDROMIC SEQUENCE, and it may lie
e.g. between the PROMOTER and the coding sequence of a gene, or
between the promoter and first structural gene in an operon or
(as in the TRP OPERON) it may occur entirely within the promoter
region.
Oocystis
A genus of unicellular, non-motile, ellipsoidal or
lemon-shaped, freshwater green algae (division CHLOROPHYTA);
asexual reproduction occurs by autospore formation.
Oodinium See DINOFLAGELLATES and VELVET DISEASE.
oogamy Fertilization involving morphologically distinguishable
male and female elements typically a large non-motile female
gamete and a small motile male gamete (see e.g. MONOBLEPHARIDALES; cf. OOMYCETES). (See also ANISOGAMY.)
oogonium A female structure in which one or more gametes
(oospheres) develop; a fertilized oosphere is called an oospore.
ookinete A motile zygote.
Oomycetes A class of aquatic and terrestrial fungi (subdivision
MASTIGOMYCOTINA) which typically give rise to zoospores having one anteriorly-directed tinsel flagellum and one posteriorlydirected whiplash flagellum (cf. PERONOSPORA). The organisms
include saprotrophs and parasites the latter including some
important pathogens of cultivated crops. According to species,
the thallus ranges from a simple, unicellular, holocarpic structure to a well-developed mycelium; in at least some species the
thallus is diploid. The CELL WALL is generally believed to lack
chitin and to contain CELLULOSE; however, there is evidence that
CHITIN and cellulose both occur in the wall in e.g. certain members of the LEPTOMITALES and Saprolegniales. Some oomycetes
exhibit DIPLANETISM, others MONOPLANETISM. Sexual reproduction is oogamous, involving the fusion of non-motile male and
female elements within gametangia (cf. MONOBLEPHARIDALES).
Orders: LAGENIDIALES, LEPTOMITALES, PERONOSPORALES, SAPROLEGNIALES.
Some authors include this class of fungi in the subdivision
Diplomastigomycotina of the division Mastigomycota.
oophoritis Inflammation of the ovaries.
oosphere See OOGONIUM.
oospore See OOGONIUM.
Oosporidium
A genus of non-fermentative imperfect yeasts
(class HYPHOMYCETES). The cells are variously shaped, reproduce by multilateral bud-fission, and usually remain attached to
each other to form long chains. Asexual endospores are formed,
arthrospores are not. Pink or orange-yellow non-carotenoid pigments are synthesized. One species: O. margaritiferum, isolated
from the slime flux of trees. [Book ref. 100, pp. 886889.]
Opa proteins (of Neisseria) In pathogenic strains of Neisseria:
OUTER MEMBRANE adhesins, encoded by opa genes, whose
presence affects the opacity (hence Opa) and colour of the
colonies (owing to increased bacterial aggregation); the Opa
proteins mediate adhesion to (and uptake by) epithelial cells or
opsonin-independent phagocytosis by PMNs. (Non-pathogenic
strains of Neisseria contain genes with sequences homologous
to those of the opa genes; it is possible that the products of
these genes may mediate mucosal colonization by commensal
strains.) (See also CD66.)
Some Opa+ strains exhibit TRANSCYTOSIS.
Within a given cell, the chromosome contains several allelic
(variant) forms of opa gene, and the organisms exhibit phase
variation, i.e. a given cell may change (e.g.) from expressing a
single type of opa gene to expressing more than one type (or
no type) of opa gene. Phase variation is regulated by certain
DNA re-arrangements in the 5 leader sequence of the opa
genes. The 5 region of these genes contains multiple copies
of a pentameric sequence (CTCTT), and the number of copies
of this coding repeat can vary; thus, while all the opa genes are
transcribed constitutively, translation of a transcript will give rise
to a functional Opa protein only if the number of (pentameric)
coding repeats is such that the coding sequence of the gene is
in the correct reading frame.
537
Opercularia
In operons under negative promoter control, the binding of
repressor to operator sequence(s) inhibits initiation of transcription. The gal operon (encoding utilization of galactose, and
biosynthesis of UDP-galactose) contains two operators (located
on either side of the promoter region); it appears that, in the
repressed state, these two sequences may be physically linked
by an oligomer of the repressor protein (GalR) to form a DNA
loop that (by sequestering the promoter region) inhibits initiation
of transcription. (See also LAC OPERON.) Such DNA looping is
also used for transcriptional control in the araBAD operon (see
ARA OPERON). This operon contains four operator sequences, and
the way in which the regulatory protein (AraC) binds to particular sequences (influenced by the presence/absence of arabinose)
controls the activity of the araBAD operon. When arabinose is
absent, AraC binds to the I1 and O2 operators, forming a loop
that represses transcription. In the presence of arabinose, the arabinoseAraC complex binds to the I1 and I2 operators (which
are close together and also referred to, jointly, as the initiator,
araI ); this promotes transcription of araBAD.
In Pseudomonas aeruginosa, synthesis of the siderophore
PYOVERDIN is apparently controlled by a transcriptional regulator,
the FUR PROTEIN, via an operator designated the Fur box
or iron box; with adequate iron, Fur binds to the operator,
blocking transcription of pvdS a gene encoding a SIGMA
FACTOR necessary for the synthesis of pyoverdin [see JB (1996)
178 22992313].
Iron-regulated transcriptional control occurs at the operator
of the tox gene encoding diphtheria toxin. Repression of tox by
transitional metal ions apparently involves a helix-to-coil change
in the repressor protein (DtxR); in this (iron-modified) state,
dimers of DtxR inhibit transcription by binding on either side of
the operator region [Nature (1998) 394 502506].
Opercularia
A genus of sedentary ciliate protozoa (subclass
PERITRICHIA) which occur in various freshwater habitats; some
species (e.g. O. coarctata) are common in SEWAGE TREATMENT
plants. Opercularia resembles CARCHESIUM, but the zooid lacks
a flared rim, and the stalks are non-contractile.
operculate ascus An ASCUS whose wall has a large, annular,
apical thickening that encloses a circular region of thinner wall
tissue; the circular region of tissue ruptures prior to ascospore
discharge.
operculum (mycol.) A hinged lid or an easily detachable portion
of the wall in a sac-like spore-bearing structure (see e.g.
OPERCULATE ASCUS).
operon In prokaryotes: two or more genes whose expression can
be co-ordinated from (i) a common PROMOTER, the contiguous
genes being transcribed as a single polycistronic mRNA (see
e.g. LAC OPERON) or (ii) a common regulatory region mRNAs
being formed by DIVERGENT TRANSCRIPTION from different promoters.
The genes in an operon are often though not necessarily functionally related: e.g. they may encode enzymes of a
particular metabolic pathway. The organization of genes into an
operon may allow their expression to be co-ordinately turned
on (induced ) or turned off (repressed ) according to the cells
needs. For example, enzymes of a catabolic pathway may be
induced in the presence of the substrate of that pathway, and
repressed again when the substrate has been used up; enzymes
of an anabolic pathway must be induced when the end-product
of the pathway becomes limiting and repressed when adequate
levels of the product have been synthesized. Regulation of structural gene expression may occur at the level of transcription
initiation (promoter control ), transcription termination (attenuator control ), or a combination of both; exceptionally, regulation
occurs at the level of translation.
Promoter control. An operon under promoter control is
commonly regulated by the product of a specific regulator gene
which may or may not be contiguous with the structural genes.
(Opinions differ as to whether or not the regulator gene should
be regarded as part of the operon.) The regulator gene generally
has its own promoter and may be expressed constitutively or
may be subject e.g. to AUTOGENOUS REGULATION. The operon
is said to be under negative control if the structural genes are
expressed until turned off by the regulator protein, and under
positive control if they are not expressed until turned on by the
regulator protein. (The regulator protein may require a low-MWt
effector molecule for activity.)
In a negatively controlled operon the regulator gene encodes
a repressor protein which binds to a specific region of the
DNA (the OPERATOR) upstream of the structural genes, thereby
preventing the initiation of transcription. If the structural genes
encode enzymes of a catabolic pathway, the presence of the
substrate brings about the induction of gene expression. The
molecule effecting induction is called an inducer; it is not
necessarily the substrate of the pathway itself, but may be e.g.
a derivative of it. (Certain analogues of the natural inducer may
also act as inducers; an analogue which can act as an inducer but
which cannot be metabolized by the cell is called a gratuitous
inducer.) The inducer inactivates the repressor, causing it to
release the operator and allow transcription to proceed. When
the substrate is removed (e.g. when all of the substrate has
been metabolized) the repressor again binds to the operator
and transcription ceases; since mRNA is generally short-lived
in bacteria (see MRNA), enzyme synthesis also rapidly ceases.
(See e.g. LAC OPERON.)
Structural genes encoding enzymes involved in an anabolic
pathway may also be subject to negative control. In this case,
the regulator gene encodes an aporepressor which cannot itself
bind to the operator of the operon, but which can do so when
it interacts with the end-product of the pathway (or a derivative
or analogue of it), the corepressor.
In a positively-controlled operon the regulator protein may
be an activator (= inducer protein) which binds to a region
of the operon (the initiator ), thereby turning on (activating)
transcription initiation. In the case of a catabolic operon the
regulator gene may encode an apo-activator which must interact
with the substrate (or a derivative of it), the co-activator, to form
a functional activator. (See e.g. ARA OPERON.)
Attenuator control. Attenuation is a regulatory mechanism in
which gene expression is prevented by the termination of transcription at a rho-independent terminator (see TRANSCRIPTION),
the attenuator, in the LEADER region of the mRNA; thus, transcription is terminated before the RNA polymerase reaches the
first structural gene of the operon. Whether or not transcription
terminates at the attenuator depends on the secondary structure
adopted by the leader region of the mRNA: in one conformation
the stem-and-loop structure of the rho-independent terminator
is formed and transcription is terminated, while in the alternative conformation the terminator structure is not formed and
transcription continues into the structural genes.
Attenuation is involved e.g. in the regulation of various
operons concerned with amino acid biosynthesis. In these
operons the leader encodes a small peptide which contains a
relatively high proportion of the amino acid whose biosynthesis
is encoded by the operon. If the amino acid is present at levels
538
by Neisseria gonorrhoeae (see GONORRHOEA) or Chlamydia trachomatis. (The disease caused by C. trachomatis is also called
inclusion blennorrhoea or inclusion conjunctivitis.) [Chlamydial ophthalmia neonatorum (aetiology, epidemiology, diagnosis,
prophylaxis and treatment): Book ref. 193, pp. 297304.]
opine See CROWN GALL.
opisthe (ciliate protozool.) The posterior of the two cells formed
during HOMOTHETOGENIC cell division. (cf. PROTER.)
opisthomastigote See HERPETOMONAS and TRYPANOSOMATIDAE.
oppBCDF genes See PEPTIDOGLYCAN.
opportunist pathogens Organisms which are normally freeliving, or which occur as part of the normal body flora, but which
may adopt a pathogenic role under certain conditions e.g.
when the normal antimicrobial defence mechanisms of the host
have become impaired; thus, e.g. Bacteroides spp (common
inhabitants of the human gut) may give rise to peritonitis
following bowel surgery. (See also ENDOGENOUS INFECTION.)
opsin The apoprotein of e.g. BACTERIORHODOPSIN (bacterioopsin), HALORHODOPSIN (halo-opsin) or SLOW-CYCLING RHODOPSIN
(slow-opsin).
opsonic index The ratio of phagocytic activity of a patients
blood to that of a normal (non-immune) subject in respect of a
specific opsonin. To determine the opsonic index: both (citrated)
blood samples are incubated for 15 min with a standard number
of the relevant antigenic particles (usually microbial cells); the
average number of particles engulfed by the phagocytes is then
determined by microscopy of smears from each sample the
ratio of the two averages being the opsonic index.
opsonin Any molecule which, when combined with a particulate
antigen, increases the susceptibility of that antigen to PHAGOCYTOSIS. Opsonins include: (i) certain types of antibody (e.g.
most types of IgG) receptors for the FC PORTION of an antibody occurring e.g. on the macrophage surface; (ii) the C3b
and C4b components of COMPLEMENT; (iii) certain ACUTE-PHASE
PROTEINS.
opsonization The process in which a particulate antigen (e.g. a
microbial cell) becomes more susceptible to PHAGOCYTOSIS as
a result of combination with an OPSONIN. The term may refer
to either a complement-dependent or complement-independent
increase in susceptibility.
optical bleach Syn. FLUORESCENT BRIGHTENER.
optical brightener Syn. FLUORESCENT BRIGHTENER.
optical density See TURBIDIMETRY.
optical staining Syn. RHEINBERG ILLUMINATION.
optimal proportions (optimal ratio; equivalence) (serol.) In a
PRECIPITIN TEST: the proportions in which antigen and antibody
must be mixed in order to obtain the maximum amount of precipitate; for a given antigenantibody system different optimal
proportions are observed in the DEAN AND WEBB TITRATION and the
RAMON TITRATION. (See also ANTIGEN EXCESS and LATTICE HYPOTHESIS.)
optochin Ethylhydrocupreine hydrochloride (EHC): a reagent
which strongly inhibits the growth of Streptococcus pneumoniae;
other streptococci which form colonies similar to those of
S. pneumoniae are commonly resistant to ten or more times the
concentration of optochin that inhibits S. pneumoniae. Optochin
is used to detect the presence of S. pneumoniae in a mixed flora;
the sample is streaked onto the surface of a solid medium, and
an optochin-impregnated paper disc is placed on the medium
prior to incubation. A significant decrease in the number of
colonies in the vicinity of the disc may indicate the presence
of S. pneumoniae.
oral hairy leukoplakia See HAIRY LEUKOPLAKIA.
539
oral herpes
although changes in pH may also affect e.g. transport systems
and/or surface properties in the target cells. In membrane
vesicles of Escherichia coli, parabens and sorbic acid were found
to eliminate 1pH leaving 1y much less disturbed [JGM
(1985) 131 7376].
organism See MICROORGANISM.
organoleptic Affecting the organs of sense particularly those
of taste and smell.
organophosphorus compounds Phosphorus-containing organic
compounds are widely used as insecticides and acaricides,
and some are also effective agricultural ANTIFUNGAL AGENTS;
the latter include e.g. ditalimfos (used against barley powdery
mildew), HINOZAN, KITAZIN, and PYRAZOPHOS. [Accumulation,
metabolism and effects of organophosphorus insecticides on
microorganisms: AAM (1982) 28 149200.]
organotin See TIN.
organotroph An organism which obtains energy by the
metabolism of an organic substrate (i.e., a chemoorganotroph)
or which uses an organic substrate as an electron donor
in phototrophic metabolism (i.e. a photoorganotroph). (cf.
LITHOTROPH; HETEROTROPH.) Chemoorganotrophs may obtain
energy from organic substrates e.g. by FERMENTATION (sense 1)
and/or by RESPIRATION; substrates may include any of a wide
range of compounds, e.g. (depending on species) various
sugars, amino acids, fatty acids, cyclic compounds, etc.
Photoorganotrophs include e.g. certain photosynthetic bacteria
which use relatively simple substrates (e.g. acetate, caproate,
lactate) as electron donors in PHOTOSYNTHESIS.
orgmet See BIOMIMETIC TECHNOLOGY.
ori
A designation which usually indicates an origin of DNA
REPLICATION (see e.g. oriC ); oriT is an origin of transfer (see
CONJUGATION sense 1b).
ori1 See F PLASMID.
ori2 See F PLASMID.
oriC An origin of chromosome replication. In Escherichia coli
the oriC region is ca. 245 bp long and contains sequences
for recognition by and interaction with initiation factors;
these sequences are precisely separated by spacer sequences
[Book ref. 69, pp. 257273; interaction of oriC with proteins:
pp. 289301]. (See also DNA REPLICATION.)
oriental sore See CUTANEOUS LEISHMANIASIS.
origin (mol. biol.) See DNA REPLICATION.
oriS See F PLASMID.
orisome See DNA REPLICATION.
oriT See CONJUGATION (1b) (i).
oriV The/an origin of vegetative replication in a PLASMID. (cf.
oriT in CONJUGATION (1b) (i).)
Orleans process See VINEGAR.
ornidazole See NITROIMIDAZOLES.
L-ornithine See e.g. Appendix IV(a).
ornithine carbamoyltransferase See ARGININE DIHYDROLASE and
Appendix IV(a).
ornithine decarboxylase test See DECARBOXYLASE TESTS.
Ornithocercus A genus of tropical marine DINOFLAGELLATES in
which the cells have elaborate thecal extensions (wings).
ornithocoprophilous Preferring a habitat rich in bird faeces.
ornithosis See PSITTACOSIS.
orotate Uracil 4-carboxylate: see Appendix V(b).
orotidine monophosphate See Appendix V(b).
Oroya fever See BARTONELLOSIS.
orphan virus A virus which is not known to cause any disease.
orseille Syn. ORCHIL.
Orthocerina See FORAMINIFERIDA.
osmoregulation
osmic acid See OSMIUM TETROXIDE.
osmiophilic Having an affinity for OSMIUM TETROXIDE.
osmium tetroxide (osmic acid; OsO4 ) A volatile compound
used e.g. for post-FIXATION (12% w/v in phosphate or cacodylate buffer); the specimen is immersed in (or exposed to the
vapour of) the solution. OsO4 may cross-link and stabilize
e.g. lipids by reacting with their double bonds. Longer exposure to OsO4 may be used for positive staining in ELECTRON
MICROSCOPY.
osmolyte Syn. OSMOTICUM.
osmophilic Refers to an organism which grows optimally in or
on media of high osmotic pressure.
osmoregulation A form of ADAPTATION in which a cell increases
or decreases its intracellular osmotic pressure in response to
an increase or decrease, respectively, in extracellular osmotic
pressure. Maintenance of internal osmotic pressure, within
certain limits, is necessary for growth/viability; for example,
osmotic withdrawal of water from a cell without adaptive
response would tend to raise the concentrations of some
solutes to levels that may be inhibitory or lethal.
In microorganisms osmoregulation involves the regulation of
intracellular concentrations of certain types of solute and/or (in
some eukaryotes) the action of CONTRACTILE VACUOLES.
Solutes used in osmoregulation include certain ions (e.g.
K+ ) and a number of low-MWt organic compounds such
as glutamate and glycine betaine ((CH3 )3 .N+ .CH2 COO ), a
substance common in nature. (See also COMPATIBLE SOLUTE.)
Solutes (osmotica) may be taken up from the environment
and/or synthesized in situ. Uptake or pumping out of ions
through the cytoplasmic membrane involves e.g. the activity
of particular types of ATPase; this form of osmoregulation is
common in bacteria: see e.g. the Escherichia coli Kdp-based
system in TWO-COMPONENT REGULATORY SYSTEMS. Another form
of osmoregulation in E. coli is controlled by a different twocomponent system. In this system, increased osmolarity in the
environment stimulates the kinase activity of a cell-envelope
sensor, EnvZ, which transfers phosphate to the regulator protein,
OmpR; activated OmpR (i) enhances transcription from ompC
(the gene encoding OmpC PORIN) and (ii) inhibits transcription
from the OmpF porin gene. Hence, increased osmolarity results
in a modified outer membrane containing a higher proportion of
OmpC (which forms a pore smaller than that of OmpF).
Following osmotic up-shift, uptake of glycine betaine is
common in both Gram-positive and Gram-negative bacteria. In
E. coli this compatible solute is taken up very efficiently by
a binding-protein-dependent transport system (a so-called ABC
importer) designated ProU [FEMS Reviews (1994) 14 320].
The bacterium Sinorhizobium meliloti actually metabolizes
most of the known osmoprotectants, including glycine betaine; in
S. meliloti, osmotic up-shift triggers the accumulation of endogenous solutes (e.g. glutamate and N-acetylglutaminylglutamine
amide) accumulation being stimulated e.g. by exogenous
sucrose [JB (1998) 180 50445051].
[Regulation of compatible solute accumulation in bacteria:
Mol. Microbiol. (1998) 29 397407.]
Osmotic down-shift triggers efflux systems. For example, K+
ions and glutamate are released rapidly by E. coli (efflux apparently being energy-independent); much of the K+ released is
believed to pass through mechanosensitive channels in the CYTOPLASMIC MEMBRANE: stretch-activated channels which respond to
increases in the cells turgor pressure by increasing their pore
size [JBC (1997) 272 3215032157]. In some bacteria (including E. coli ) the membrane contains structures called aquaporins
that may contribute to osmoregulation.
osmotic shock
osteosarcoma See SARCOMA.
ostiole (mycol.) A tubular or pore-like opening to the exterior in
e.g. a perithecium, pseudoperithecium or pycnidium.
Ostracoblabe implexa
A coenocytic, mycelial fungus (taxonomic position uncertain) which occurs on the shells of marine
molluscs, obtaining nutrients from the organic matrix of the
shell. In the European flat oyster (Ostrea edulis) the fungus
causes shell disease: it penetrates between the shell and mantle of the oyster, causing severe irritation; the oyster responds
by producing a highly proteinaceous shell which further encourages growth of the fungus. Shell disease occurs mainly in shallow waters where temperatures commonly exceed 18 C. [Book
ref. 1, pp. 216218.] (See also OYSTER DISEASES.)
Ostreobium
A genus of siphonaceous green algae (division
CHLOROPHYTA) which grow endolithically in shells and corals
(and beneath the layer of zooxanthellae in corals) in tropical and
temperate oceans; the cells contain siphonein and siphonoxanthin, and their photosynthetic pigments have absorption maxima
in the far-red.
ostreogrycins See STREPTOGRAMINS.
ostropalean ascus An ASCUS whose wall contains a substantial,
non-refractive apical thickening (apical cap); at maturity, the
ascospores are discharged via a narrow channel in the cap. Such
asci characteristically contain filiform ascospores.
Ostropales An order of saprotrophic, plant-parasitic and lichenized fungi of the ASCOMYCOTINA. Ascocarp: apothecioid or perithecioid. Asci: unitunicate, inoperculate, cylindrical. Ascospores:
commonly filiform.
OT Old TUBERCULIN.
Oth-25/89/J virus A SMALL ROUND STRUCTURED VIRUS.
otitis media Inflammation of the middle ear. The condition is
commonly suppurative: pyogenic bacteria from the throat infect
the middle ear via the eustachian tube often following an
upper respiratory tract infection or tonsillitis. The eustachian
tube becomes blocked, and pus formation causes bulging and
sometimes rupture of the eardrum. Causal agents include e.g.
Haemophilus influenzae, Moraxella (Branhamella) catarrhalis,
Streptococcus pneumoniae and S. pyogenes.
otomycosis A MYCOSIS affecting the ears (see e.g. ASPERGILLOSIS).
Ottens antigens Polysaccharide antigens which occur in many
strains of Streptococcus milleri but which seldom occur in other
streptococci.
OTU Operational taxonomic unit: a designation applied to each
individual strain, species, genus etc used in classification carried
out by NUMERICAL TAXONOMY; in bacteriology OTU commonly
refers to a given strain.
ouabain (g-strophanthin) A polycyclic, L-rhamnose-containing
glycoside which inhibits Na+ /K+ -ATPase (see ION TRANSPORT).
Ouchterlony test A GEL DIFFUSION test of the DOUBLE DIFFUSION,
double DIMENSION type. A pattern of holes (wells) is cut into a
sheet of agar (or similar material) contained (e.g.) in a Petri dish.
The number and arrangement of wells depend on the number and
nature of the samples to be tested, and on the purpose of the test.
Each well is filled with an antigen, antibody (usually antiserum),
or control preparation; the whole is covered (to prevent drying)
and incubated (usually at room temperature) for hours or (more
usually) days. The diagram shows the arrangement of wells,
and some possible results, for the serological comparison of two
samples of antiserum.
Oudemansiella See AGARICALES (Tricholomataceae).
Oudin test See SINGLE DIFFUSION.
out genes See PROTEIN SECRETION (type II systems).
outer envelope See SPIROCHAETALES.
outer membrane
Ag
Ag
Aga
X
Agb
Aga
Agc
Ab
Ab
AbaAbc
(a)
(b)
(c)
OUCHTERLONY TEST. (a) Reaction of identity. With wells located symmetrically, the lines of precipitate are symmetrical and do not
overlap. Since the antigens (Ag) in the top two wells react identically with the antibody (Ab) they are taken to be serologically identical.
(b) Reaction of partial identity. X is a line of precipitate formed where antibody and its homologous antigen (Aga ) meet in optimal proportions.
At Y, antibody and a cross-reactive antigen (Agb ) meet in optimal proportions. In this instance, Agb has less affinity than Aga for the antibody,
and antibody which has diffused beyond Y forms a precipitate with Aga at Z; Z, which is called a spur, points towards the cross-reactive
antigen. (c) Reaction of non-identity. Two independent precipitating systems are present: each antibody reacts only with its homologous
antigen.
Oxymonadida
of the medium). Acidification in only the uncovered medium
indicates oxidative attack on the carbohydrate, while acidification in the covered tube indicates that the carbohydrate can be
attacked fermentatively; no reaction in either tube usually indicates that the particular carbohydrate is not utilized by the test
organism. [Modified medium for marine bacteria: AEM (1985)
49 15411543.]
oxidationreduction potential REDOX POTENTIAL.
oxidative metabolism See RESPIRATION.
oxidative pentose phosphate pathway Syn. HEXOSE MONOPHOSPHATE PATHWAY.
oxidative phosphorylation As commonly used: the phosphorylation of ADP to ATP, or the formation of PYROPHOSPHATE from
inorganic phosphate, in a reaction which is driven by energy
derived from proton motive force (see CHEMIOSMOSIS) generated by means of a respiratory chain; electron transport may
be driven by aerobic RESPIRATION or by ANAEROBIC RESPIRATION.
Oxidative phosphorylation may be catalysed by a PROTON ATPASE
or a PROTON PPASE. (cf. ELECTRON TRANSPORT PHOSPHORYLATION
and SUBSTRATE-LEVEL PHOSPHORYLATION.)
oxidative rancidity RANCIDITY due to AUTOXIDATION of a foods
unsaturated fatty acids; such oxidation is encouraged e.g. by
metal ions and by light. The occurrence of oxidative rancidity
can be inhibited or delayed e.g. by refrigeration, by removing
oxygen (e.g. by vacuum packing), or by the use of ANTIOXIDANTS.
oxidizing agents (as antimicrobial agents) Strong or moderately
strong oxidizing agents can behave as effective antimicrobial
agents when they are present in adequate concentrations under
suitable conditions. However, their use as DISINFECTANTS is
often limited by their high reactivity which renders them
liable to inactivation in the presence of excess organic matter.
Inactivation by inert organic matter can be compensated for by
using a concentration of the oxidizing agent sufficient to oxidize
the inert matter and to leave a residual concentration which can
act against viable microorganisms see e.g. chlorine demand in
WATER SUPPLIES. (For adaptation of bacteria to oxidizing agents
see HYDROGEN PEROXIDE.)
Antimicrobial oxidizing agents include e.g. CHLORINE, HYDROGEN PEROXIDE, HYPOCHLORITES, OZONE and POTASSIUM PERMANGANATE.
oxidoreductases ENZYMES (EC class 1) which catalyse oxidationreduction reactions. (See also DEHYDROGENASE; OXIDASE;
OXYGENASE; PEROXIDASE.)
oxine Syn. 8-HYDROXYQUINOLINE.
Oxobacter See CLOSTRIDIUM.
2-oxoglutarate dehydrogenase See TCA CYCLE.
oxolinic acid An analogue of NALIDIXIC ACID; it resembles
nalidixic acid in its mode of action but is much more potent.
6-oxo-PGF1a See PROSTACYCLIN.
oxycarboxin See CARBOXIN.
Oxyfume Sterilants A range of STERILANTS containing ETHYLENE
OXIDE.
oxygenase An OXIDOREDUCTASE which catalyses the incorporation of one or both atoms of a molecule of oxygen into a
molecule of substrate. A MONOOXYGENASE catalyses the incorporation of one atom of oxygen, the other being reduced to water;
a dioxygenase (EC 1.13.11) catalyses the incorporation of both
atoms of oxygen. Oxygenases are frequently involved e.g. in the
first step of the bacterial degradation of HYDROCARBONS.
oxygenic photosynthesis See PHOTOSYNTHESIS.
oxyhydrogen reaction KNALLGAS REACTION.
Oxymonadida An order of protozoa (class ZOOMASTIGOPHOREA)
which are parasitic in insects (e.g. termites). Cells have one
Oxymonas
(cf. SHII-TAKE); oyster fungi have also been grown on a number
of waste materials such as sawdust, cereal straws, cotton waste,
waste paper etc. [Mycol. (1983) 75 351360.]
ozaena (ozena) Rhinitis, caused by Klebsiella pneumoniae subsp
ozaenae, characterized by a profuse, mucopurulent, fetid nasal
discharge with crusting of the nasal mucosa.
ozena Syn. OZAENA.
ozone (as an antimicrobial agent) Ozone (O3 ) is an OXIDIZING
AGENT which reacts readily with most types of organic matter
and which is active against a wide range of microorganisms; it
is more efficient at lower temperatures, and requires a minimum
relative humidity of ca. 60% for the disinfection of surfaces.
Ozone has been used for the preservation of certain foods, but it
is active against only surface contaminants, and it is not suitable
for use with fats, meat etc which are likely to be oxidized. Ozone
is sometimes used for the disinfection of potable WATER SUPPLIES;
for this purpose it is superior to chlorine in that it is a stronger
oxidizing agent, it is less affected by pH, and it does not impart a
taste or odour. The treatment of wastewater (processed sewage)
with ozone, rather than with chlorine, is advantageous e.g. in
that it avoids the production of possibly toxic chlorinated organic
compounds. The disinfection of water by ozone has been studied
by monitoring the consumption of ozone-generated hydroxyl free
radicals [Wat. Res. (1984) 18 473478]. (See also INFLUENZA.)
PARTICLE.
AN
oxysome Syn. FERNANDEZMOR
oxysporum wilt See FUSARIUM WILT.
oxytetracycline See TETRACYCLINES.
Oxytricha See HYPOTRICHIDA.
oyster cap Syn. OYSTER FUNGUS.
oyster diseases For pathogens of oysters (e.g., Ostrea and Crassostrea spp) see e.g. LAGENIDIALES; MINCHINIA; OSTRACOBLABE
IMPLEXA; PERKINSUS; VAHLKAMPFIA; VIBRIO (e.g. V. anguillarum).
(See also INVERTEBRATE DISEASES.)
oyster fungus (oyster mushroom or oyster cap) Any species of
Pleurotus, but especially P. ostreatus. A number of Pleurotus
spp are edible and can easily be cultivated by inoculating logs
546
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
P
p
RETROVIRIDAE).
547
paired organelles
its solvent. Liquid emulsion paints may contain a variety of
organic substances (e.g. as stabilizers, thickeners), inorganic constituents, and a high content of water, and may be susceptible
to attack by bacteria (e.g. Pseudomonas spp) and fungi (e.g.
Fusarium spp); biocides incorporated in such paints (to extend
shelf-life) include e.g. organo-tins (such as tributyl tin oxide),
certain QUATERNARY AMMONIUM COMPOUNDS, and mercurials such
as phenylmercuric acetate. Oil-based liquid paints are less susceptible to spoilage, but the hardened films of both oil-based
and emulsion paints are susceptible to attack particularly under
humid conditions and when surfaces are soiled; spoilage organisms may obtain nutrients from the film itself, from surface
contamination, or from the substrate (wood etc) beneath the film.
Spoilage organisms include species of the fungi Aspergillus,
Aureobasidium, Cladosporium and Penicillium; cyanobacteria
(e.g. Nostoc, Oscillatoria) and algae (e.g. Trentepohlia) may
grow given adequate moisture and light. Biocides are incorporated in paints to help paint films resist microbial attack; these
include e.g. organo-mercury compounds, SALICYLANILIDES, halogenated phenolics, and a variety of copper and zinc compounds.
Antifouling paints are used e.g. on ships hulls to inhibit
both spoilage and colonization by microorganisms and other
organisms. In soluble-matrix paints the binder constituent is
(slowly) soluble in seawater, low levels of biocide continually
becoming available at the surface. In other paints, biocide
diffuses slowly to the surface of an insoluble matrix. Biocides
used include e.g. copper and zinc compounds, phenols and
dithiocarbamates; some (e.g. tributyl tin oxide) inhibit algae as
well as fungi.
paired organelles Syn. RHOPTRIES.
paired sera Two samples of serum from a given patient the
second sample taken e.g. days or weeks after the first. Paired
sera are used e.g. to monitor changes in antibody titres.
Palade pathway In a eukaryotic cell: the path followed by many
types of protein from their site of synthesis to their final cellular
or extracellular location. Thus, e.g., a protein destined for secretion is synthesized on a ribosome bound to the cytoplasmic face
of the rough ENDOPLASMIC RETICULUM (RER); it is translocated
to the luminal face of the RER (see SIGNAL HYPOTHESIS) and is
then enclosed within a vesicle (cisterna) which buds from the
smooth endoplasmic reticulum and subsequently coalesces with
a vesicle in the GOLGI APPARATUS. Finally, a secretory vesicle
(containing the protein) buds from the Golgi apparatus and subsequently fuses with the cytoplasmic membrane to release the
protein at the cell surface. Other types of protein e.g. those
destined for the cytoplasmic membrane itself, or for the lumen
of a LYSOSOME follow an analogous pathway; additionally, in
cells infected with certain enveloped viruses the viral ENVELOPE
proteins are transported to their appropriate membrane via this
pathway. The production of secretory vesicles at the Golgi apparatus, and the subsequent fusion of these vesicles with the cytoplasmic membrane, can be inhibited e.g. by MONENSIN which
can therefore inhibit the replication of certain viruses.
Characteristically, proteins become progressively more glycosylated during their passage along the Palade pathway, and their
intracellular location may even by determined by their degree of
glycosylation. The glycosylation of newly synthesized (cell or
viral) proteins may be inhibited e.g. by TUNICAMYCIN.
Proteins that are not transported via the Palade pathway
include e.g. the small subunit of ribulose-1,5-bisphosphate carboxylaseoxygenase. This protein is synthesized (with an Nterminal signal peptide) on a cytoplasmic (i.e., not membranebound) ribosome and is taken up, post-translationally, by chloroplasts being proteolytically processed during or after uptake.
papilloma
PAP technique (peroxidaseantiperoxidase technique) An IMMUNOPEROXIDASE METHOD which involves three antibody-mediated
stages. Initially, separate antisera are raised (e.g. in rats) against
(i) the specific antigen and (ii) a peroxidase; if these antisera
are rat-derived, anti-rat Ig antiserum is raised e.g. in a rabbit. To
locate specific antigen in a section, the section is first treated with
rat antiserum homologous to the antigen (primary antiserum)
and then washed free of uncombined antibody. The section is
then treated with excess rabbit anti-rat Ig antiserum; under such
antiserum-excess conditions, rabbit anti-rat Ig antibodies tend to
bind to rat antibodies with only one of their combining sites.
The section is washed and then treated with rat anti-peroxidase
antiserum these antibodies being bound by the free combining sites of the rabbit anti-rat Ig antibodies. (The rabbit anti-rat
Ig antibodies are called bridging or linking antibodies.) Peroxidase is then added and combines with rat anti-peroxidase.
Peroxidase (and hence antigen) is detected by incubating the
section with reagents as in the ABC IMMUNOPEROXIDASE METHOD.
papain A heat-stable, basic thiol PROTEASE (EC 3.4.22.2) obtained
from the latex and unripe fruit of the pawpaw (Carica papaya).
(See also IMMUNOGLOBULINS.)
Papaya mosaic virus See POTEXVIRUSES.
Papaya ringspot virus See POTYVIRUSES.
PapB See P FIMBRIAE.
paper partition chromatography See CHROMATOGRAPHY.
paper spoilage Pulpwood (timber selected for pulping) may be
attacked e.g. by cellulolytic fungi such as Poria and Stereum
(see also TIMBER SPOILAGE). Wood pulp (produced from pulpwood by mechanical or chemical methods) is a watery suspension containing e.g. cellulose, hemicelluloses, sugars and
proteins; it is susceptible to attack by a range of cellulolytic
fungi (e.g. species of Aspergillus, Cladosporium, Fusarium,
Phoma and Stereum) and fungi which cause darkening or staining (e.g. species of Aureobasidium, Paecilomyces and Penicillium). Chemically prepared pulps e.g. those containing
acidified Ca(HSO3 )2 (acid sulphite pulps) or NaOH and Na2 SO3
(kraft pulps) are generally less susceptible to spoilage than are
mechanically prepared pulps. Cellulolytic attack on either pulpwood or pulp shortens the cellulose fibres, resulting in inferior
(weaker) paper. Slime formation in pulps is due e.g. to species
of Alcaligenes, coliforms and other bacteria (Serratia forms red
slime), and to fungi such as Fusarium and Geotrichum; slime
may cause weaknesses, holes and/or discoloration in the paper.
PRESERVATIVES used in pulps include e.g. dichlorophane, pentachlorophenol, and salicylanilides; slime formation has been
controlled e.g. by chlorine and mercurials. Finished paper and
board products have a low moisture content and are subject
to fungal spoilage (particularly under high humidity) by e.g.
Chaetomium globosum, Stachybotrys atra and other cellulolytic
species; Aspergillus and Penicillium spp are common causes of
discoloration. Paper and board preservatives include e.g. copper
and zinc compounds, dichlorophane, and dithiocarbamates.
papilla A microcolony, within and visibly distinct from, a
larger colony. For example, a colony of Lac mutant cells
of Escherichia coli may contain a papilla that consists of a
subpopulation of LacC revertants; on MacConkeys agar, such
a papilla would be pink/red in a colourless colony.
papilloma (pl. papillomas or papillomata) A small tumour of
epithelial tissue (skin, mucous membranes, or glandular ducts),
caused by a PAPILLOMAVIRUS; papillomas affecting the skin are
commonly known as warts or verrucas. Papillomaviruses are
largely host-specific, and different types of papillomavirus may
cause morphologically distinct types of papilloma in a given
Pandorina
549
Papillomavirus
host. In man, papillomas are caused by human papilloma viruses
(HPVs): e.g. plantar warts, caused by HPV-1, occur on the soles
of the feet and are flat, being pressed into the dermis by the
weight of the body; genital warts (venereal warts, papillomata
acuminata, condylomata acuminata), caused by HPV-6, occur in
the anogenital region and are transmitted by sexual contact (cf.
BUSCHKELOWENSTEIN
TUMOUR and MOLLUSCUM CONTAGIOSUM).
Papillomas are usually benign, but those caused by certain
viruses can become malignant in the presence of certain cofactors e.g., certain animal papillomas can become malignant on
exposure to sunlight. (cf. EPIDERMODYSPLASIA VERRUCIFORMIS.) In
cattle, papillomas (caused by bovine papilloma virus 4) in the
oesophagus and forestomachs can become malignant if the cattle
eat bracken (Pteridium aquilinum). In humans, HPVs associated
with genital warts are believed to play a role in the development
of cancer of the genital tract (particularly of the cervix) [BMJ
(1984) 288 735737; Lancet (1986) i 573575].
Papillomavirus
A genus of viruses of the PAPOVAVIRIDAE.
Type species: cottontail rabbit (Shope) papilloma virus (CRPV)
[genomic structure: PNAS (1985) 82 15801584]; other members include human papilloma viruses (many types, designated
HPV-1, HPV-2 etc), bovine papilloma viruses (BPV-1, BPV-2
etc), and papilloma viruses infecting deer, dogs, goats, horses,
rats and sheep. Papilloma viruses can induce benign squamous
epithelial tumours of the cutaneous and mucosal epithelium of
their hosts (see PAPILLOMA). The virus can infect but not replicate in the basal cells of the epidermis or mucosa, establishing
a persistent infection in which multiple copies of the viral DNA
occur in the nucleus in the form of circular extrachromosomal
molecules; however, production of virions can occur only in the
non-dividing, differentiated squamous epithelial cells of the stratum spinosum and stratum corneum. (Since these cells cannot
be grown in culture, papilloma viruses cannot be propagated in
vitro, and molecular biological studies have depended largely on
the use of cloned viral DNA.)
Although the papillomas induced by papilloma viruses are
usually benign, certain human and animal papilloma viruses
may be involved in the development of malignant tumours; in
most of these systems infection with the papilloma virus is by
itself insufficient for malignant transformation, and additional
physical, chemical and/or biological factors are necessary for
carcinogenesis (see PAPILLOMA and EPIDERMODYSPLASIA VERRUCIFORMIS). In experimental systems, several papilloma viruses can
induce fibroblastic tumours in hamsters and can transform rodent
cells in vitro (although such cells do not produce virions). The
mechanism of transformation is unknown. In BPV-1, the presence of only a portion (69%) of the viral genome is necessary
for transformation, and the expression of viral genes is apparently necessary; BPV-1 appears to carry multiple transforming
genes [PNAS (1985) 82 10301034]. There is evidence that
viral DNA may integrate into the host chromosome in at least
some cases of malignancy e.g. integrated HPV-16 DNA has
been detected in malignant tumours of the human genital tract
[JGV (1985) 66 15151522; see also Gynecologic Oncology
(1992) 47 263266].
Papovaviridae (papovavirus group) A family of non-enveloped,
small, icosahedral DNA viruses, most of which infect mammals
(cf. BUDGERIGAR FLEDGLING DISEASE VIRUS); most or all members
can induce tumours in certain host animals. Viral DNA replication and assembly occur in the host cell nucleus. The family
contains two genera: PAPILLOMAVIRUS and POLYOMAVIRUS, distinguished on the basis of size, genome characteristics, a genusspecific antigen (detected in disrupted virions), and biological
properties.
Paramyxovirus
eyes, accompanied by regional lymphadenopathy), or in a systemic disease involving various internal organs. Lab. diagnosis:
microscopy of infected tissues; serological tests (e.g. an EIA
[SAB (1984) 22 7378]). (cf. BLASTOMYCOSIS.)
Paracoccus
A genus (incertae sedis) of aerobic, oxidasepositive, catalase-positive, Gram-negative bacteria which occur
e.g. in soil and in meat-curing brines. Cells: non-motile cocci
or rods which typically contain granules of PHB. Metabolism:
respiratory (oxidative), the terminal electron acceptor being
O2 or (in anaerobic respiration) nitrate, nitrite or nitrous
oxide. One species (P. halodenitrificans) is chemoorganotrophic
and halophilic, the other (P. denitrificans) is facultatively
chemolithotrophic and methylotrophic (see METHYLOTROPHY)
and is non-halophilic. Carbon sources include a wide range of
organic compounds. Optimum growth temperature: 2530 C.
GC%: ca. 6467. Type species: P. denitrificans.
P. denitrificans (formerly Micrococcus denitrificans). Cells
(on e.g. nutrient agar): cocci, ca. 0.50.9 m diam., or rods,
ca. 0.91.2 m in length. (See also PORINS.)
P. halodenitrificans. Cells (on e.g. nutrient agar containing 1.0
M (5.8%) NaCl): cocci, ca. 0.50.9 m diam.; cells grown in
lower concentrations of electrolyte (e.g. 0.6 M NaCl) are usually
distorted, and no growth occurs below ca. 0.5 M NaCl. Isolated
from meat-curing brines.
[Book ref. 22, pp. 399402.]
paracolon An outdated term for those enterobacteria which do
not metabolize lactose within 24/48 hours at 37 C.
paracytosis Invasive behaviour by certain pathogenic bacteria in
which the pathogen crosses a layer of (eukaryotic) cells by
passing between the cells; thus, e.g. Haemophilus influenzae
can pass between the cells of lung epithelium [paracytosis by
H. influenzae in tissue cultures of lung epithelial cells: Inf.
Immun. (1995) 63 47294737]. (See also TRANSCYTOSIS.)
paraffin metabolism See HYDROCARBONS.
paraflagellar rod Syn. PARAXIAL ROD.
paraformaldehyde (HO(CH2 O)n H) A solid, white, polymeric
form of FORMALDEHYDE which, when heated, yields gaseous
formaldehyde.
parainfluenza viruses See PARAMYXOVIRUS.
parakinetal stomatogenesis See STOMATOGENESIS.
paralytic shellfish poisoning See SHELLFISH POISONING.
paramastigote A form assumed by the cells of species of
Herpetomonas and Leishmania during certain stages in their
life cycles: see TRYPANOSOMATIDAE.
Paramecium (slipper animalcule) A genus of (typically) freshwater protozoa (order HYMENOSTOMATIDA). Cells: ovoid or elongate with uniform somatic ciliature; length varies with species:
P. aurelia is ca. 120200 m, P. bursaria ca. 90150 m,
P. caudatum ca. 180300 m, P. multimicronucleatum ca.
200300 m, and P. trichum ca. 50120 m. The buccal cavity is ventral and contains a single PARORAL MEMBRANE (D
endoral membrane), two peniculi (see PENICULUS) and a QUADRULUS. STOMATOGENESIS is buccokinetal. Many species have one
micronucleus and one macronucleus; P. aurelia has an additional micronucleus, and P. multimicronucleatum has three or
four micronuclei. The presence of two CONTRACTILE VACUOLES
is typical, and most species have large numbers of TRICHOCYSTS.
Cysts are not formed. Paramecia are said to be negatively
galvanotactic. Many strains of Paramecium contain endosymbionts: see CAEDIBACTER, HOLOSPORA, LYTICUM, PSEUDOCAEDIBACTER, TECTIBACTER; see also KILLER PARAMECIA, MU PARTICLE,
ZOOCHLORELLAE. [Endonucleobiosis in ciliates: Int. Rev. Cytol.
(1986) 102 169213.]
551
paramyxoviruses
Parapoxvirus virions are ovoid, ca. 250 160 nm (for orf
virus) to 300 190 nm (for pseudocowpox virus); the outer
surface of the virion exhibits a characteristic criss-cross pattern
in negatively stained preparations. DNA MWt: ca. 85 106 .
Haemagglutinin is not formed. Infected cells contain only B-type
inclusion bodies. Infectivity of virions can be destroyed e.g. by
heating at 5860 C for 30 min. Parapoxviruses do not produce
pocks in CAM. They can bring about NON-GENETIC REACTIVATION
of inactivated orthopoxviruses.
paraprotein Immunoglobulin produced by a neoplastic clone of
B cells. (See also MYELOMA.)
parapyle See RADIOLARIA.
Paraquat Syn. METHYL VIOLOGEN.
pararosanilin A reddish TRIPHENYLMETHANE DYE.
pararotaviruses (group B rotaviruses) Viruses which are morphologically indistinguishable from ROTAVIRUSES but which lack
the group-specific antigen common to all other known (avian
and mammalian) rotaviruses; the 11 dsRNA segments also have
a unique and characteristic electrophoretic migration pattern.
Pararotaviruses have been isolated from human stool specimens,
but their clinical significance if any is unknown.
parasexual processes (mycol.) Non-sexual processes which can
result in the formation of recombinant nuclei. The process
first reported in Aspergillus nidulans (and later found in many
ascomycetes and in some deuteromycetes and basidiomycetes)
has been called the standard parasexual process. This process
starts with the formation of a heterokaryotic cell or mycelium
(see HETEROKARYOSIS) and involves the fusion of two genetically
dissimilar haploid nuclei (in the heterokaryon) to form a
single diploid nucleus. Recombination can then occur through
mitotic crossing over i.e., the (infrequent) reciprocal exchange
of chromatid segments between homologous chromosomes
during mitotic propagation of the diploid nucleus or (e.g. in
Saccharomyces cerevisiae) predominantly by gene conversion
[MR (1985) 49 3358 (4347)]. Haploidization (the formation
of haploid progeny nuclei) involves NON-DISJUNCTION in which
there is a stepwise loss of one member of each pair of
homologous chromosomes during successive mitoses.
For the imperfect fungi parasexuality brings the advantage of
genetic recombination. The importance of parasexual processes
in nature is uncertain.
[Review: Book ref. 168, pp. 191214.]
ParaSight-F test See MALARIA.
parasitaemia (parasitemia) The presence of parasites in the
bloodstream.
parasite See PARASITISM. A parasite may be obligatorily or
facultatively parasitic; it may be host- or strain-specific or able to
parasitize a range of hosts. Parasites which remain external to the
hosts cells or tissues are called ectoparasites, while those that
live intracellularly or within tissues are called endoparasites. If
the host suffers significant harm, or is killed, through the activity
of a microbial parasite, the parasite is referred to as a PATHOGEN.
Compared to its free-living (non-parasitic) relatives, a parasite
often exhibits certain aspects of degeneracy e.g. a reduction
in, or loss of, structures, organelles, or metabolic mechanisms
involving the ingestion and digestion of food, respiration,
osmoregulation or excretion. Adaptation to the parasitic mode of
life may be regarded as a form of specialization; some parasites
are so well integrated into the economy of their hosts that they
can be cultivated in vitro only with difficulty, or not at all.
parasitism SYMBIOSIS (sense 1) in which one organism (the
PARASITE) benefits at the expense of the other (the host);
typically, the parasite obtains its nutrients from the host, and
the association is detrimental to the host. (cf. COMMENSALISM.)
552
parthenogenesis
parasitology The study of certain PARASITES: their life cycles,
ecology, transmission, etc; those parasites studied in parasitology include some which are classified as microorganisms (e.g.
amoebae, trypanosomes, malarial parasites) as well as various arthropods, helminths, etc. Pathogenic bacteria, fungi and
viruses are traditionally not included within the scope of parasitology even though they can live parasitically.
parasol ants See FUNGUS GARDENS.
parasol mushroom See LEPIOTA.
parasomal sac In many ciliates (e.g. Paramecium): a small flasklike invagination of the surface membrane near the ciliary bases,
possibly involved in pinocytosis.
Parasponia See BRADYRHIZOBIUM.
parasporal crystal See DELTA-ENDOTOXIN and MILKY DISEASE.
paratenic Refers to an alternative host (of a parasite) which
is incidental to the normal life cycle of the parasite: i.e. the
paratenic host is neither essential for nor interferes with the
completion of the parasites life cycle.
parateny (ciliate protozool.) The condition in which part(s) of
a cell have lines of kinetids arranged perpendicularly to the
longitudinal axis of the cell; parateny is characteristic of some
scuticociliates (e.g. Loxocephalus).
paratope (1) The COMBINING SITE of an antibody. (2) The site
at which a cell-surface receptor combines with an exogenous
molecule.
paratose (3,6-dideoxy-D-glucose) A sugar, first isolated from Salmonella paratyphi, which occurs in the O-specific chains of the
LIPOPOLYSACCHARIDE in certain Salmonella serotypes and which
contributes to the specificity of O antigen 2 in group A salmonellae
(see KAUFFMANNWHITE CLASSIFICATION).
paratrachoma See INCLUSION CONJUNCTIVITIS.
paratuberculosis Syn. JOHNES DISEASE.
paratyphoid fever (paratyphoid) (1) (med.) An acute infectious
disease caused by Salmonella paratyphi A, B or C. It resembles TYPHOID FEVER in modes of transmission and infection, but
symptoms are milder and are often accompanied by gastroenteritis.
(2) (vet.) Any disease (paratyphoid, salmonellosis) caused
by a serotype of Salmonella and characterized by septicaemia
(particularly in young animals) and/or enteritis. In cattle, paratyphoid is often caused by S. dublin, and sometimes e.g. by
S. typhimurium; in the acute enteric form symptoms include
fever and diarrhoea, while chronic enteritis may cause general
unthriftiness. In pigs, the causal agents include S. choleraesuis
and S. typhimurium; the acute enteric form, involving fever and
diarrhoea, is often complicated by pulmonary involvement, while
in the (usually fatal) septicaemic form there may be nervous
involvement, red-purple skin discoloration (e.g. on the ears and
abdomen), and subcutaneous petechial haemorrhages. In horses,
S. typhimurium can cause e.g. an acute febrile condition with
diarrhoea and dehydration, while in very young foals it can cause
a fatal septicaemia. An asymptomatic carrier state can occur in
cattle, pigs and (to a limited extent) horses.
Parauronema See SCUTICOCILIATIDA.
paravaccinia virus See PARAPOXVIRUS.
paraxial rod (paraflagellar rod) In the FLAGELLUM of many members of the KINETOPLASTIDA, DINOFLAGELLATES and EUGLENOID
FLAGELLATES: a filament or rod which runs, within the flagellar
membrane, parallel to the axoneme or (in the helical transverse
flagellum of a dinoflagellate) parallel to the axis of the axoneme.
[Paraxial rod in trypanosomatids: JP (1986) 33 552557.]
paracentric objectives In a given microscope: a set of objective
lenses each of which gives a field of view whose centre is
identical to that of the others. (cf. PARFOCAL OBJECTIVES.)
partial veil
Genera: DENSOVIRUS, DEPENDOVIRUS, ERYTHROVIRUS, PARVO[Cell infection: JV (2004) 78 67096714.]
Parvovirus (parvovirus group) A genus of autonomous, helperindependent viruses (family PARVOVIRIDAE) which infect vertebrates, causing important diseases in domestic and other animals; parvoviruses responsible for human diseases are classified in the genus ERYTHROVIRUS. (So-called parvovirus-like
agents associated with human food poisoning are unrelated
(ssRNA) viruses currently referred to as SMALL ROUND STRUCTURED VIRUSES.)
The type species is r-1 (D Kilham rat virus or rat virus).
Other members include e.g. Aleutian mink disease virus (see
ALEUTIAN DISEASE OF MINK), bovine parvovirus, feline parvovirus
(including the subspecies FELINE PANLEUKOPENIA VIRUS, CANINE
PARVOVIRUS, mink enteritis virus), goose parvovirus (causal agent
of a fatal hepatitis in goslings aged 830 days), H-1 virus,
LuIII virus, porcine parvovirus (an important cause of infertility,
abortion and stillbirth), and minute virus of mice (MVM).
Several parvoviruses (e.g. H-1, LuIII) were originally isolated
from cell cultures.
Most parvoviruses can agglutinate the erythrocytes (red blood
cells) of at least one species of animal. [Differences in haemagglutinating activity among strains of canine parvovirus: JGV
(1988) 69 349354.]
The autonomous parvoviruses are characterized by their need
to replicate in dividing cells, and in at least some cases (see
ERYTHROVIRUS) a virus may be highly tropic for cells in a
particular phase of the cell cycle. (The frequent association of
parvoviruses with tumours may be due to their preference for
dividing cells rather than to an oncogenic potential; in fact,
parvoviruses are reported to have anti-neoplastic potential [Book
ref. 97, pp 344345].)
In some parvoviruses the virions contain only negative-strand
DNA; in others, the virions in a given population may contain
either negative-strand or positive-strand DNA.
In autonomous parvoviruses, replication of the DNA is
believed to follow a rolling hairpin model [modified rolling
hairpin model: JV (1985) 54 171177], which is outlined below.
Replication of the single-stranded DNA genome is facilitated
by the presence of a PALINDROMIC SEQUENCE at both ends of the
strand; in B19 parvovirus (see ERYTHROVIRUS) the two terminal
palindromes are identical. Replication begins at the 30 end, where
the palindromic sequence folds back on itself to form a T-shaped
double-stranded structure; strand synthesis from the 30 terminus
gives rise to a double-stranded replicative form which extends
to the 50 terminus of the genome. (During strand synthesis, the
T-shaped structure at the 50 end is apparently opened up by
strand displacement.) The original 50 end of the genome thus
becomes paired with a newly synthesized strand that includes a
(complementary) copy of the palindrome. The palindrome in
each strand spontaneously forms a double-stranded T-shaped
structure so that the 30 end is now positioned to use the newly
synthesized strand as a template for ongoing synthesis. Strand
synthesis along this (newly synthesized) template continues
with synthesis along the original genome strand, resulting in
a double-stranded genomic dimer. Nicking at specific sites leads
to regeneration and recycling of intermediates and the formation
of progeny genomes (see reference for further details).
parvoviruses (1) Viruses of the PARVOVIRIDAE. (2) Viruses of the
genus PARVOVIRUS.
PAS (p-aminosalicylic acid) A chemotherapeutic agent which is
bacteriostatic for some Mycobacterium spp, e.g., M. tuberculosis; it is used, together with e.g. ISONIAZID, in the treatment
VIRUS.
554
Pasteurella
of TUBERCULOSIS. PAS is incorporated in FOLIC ACID (in place of
PABA), giving rise to an analogue with impaired activity.
PAS reaction (periodic acidSchiff reaction) A procedure for
demonstrating the presence of certain carbohydrates e.g. CELLULOSE, GLYCOGEN, STARCH. Adjacent hydroxyl groups in the
carbohydrate are oxidized to aldehyde groups by periodic acid
(HIO4 ); the aldehyde groups react with SCHIFFS REAGENT to give
a purple coloration. (Tetraacetic acid or chromic acid may be
used in place of periodic acid.) A positive PAS reaction is also
given by sugars containing an unsubstituted amino group adjacent to a hydroxyl group (as in CHITOSAN). The PAS reaction has
been used e.g. to detect certain pathogenic fungi (e.g. Blastomyces dermatitidis, Histoplasma capsulatum) in tissue sections.
pascal (Pa) The SI unit of pressure; 1 pascal is equal to
1 newton/metre2 . 1 mmHg D 1 torr D 133.3 Pa D 0.133 kPa.
(1 atmosphere D 14.7 lb/inch2 D 101.325 kPa.) (cf. BAR.)
paspalinines See PASPALUM STAGGERS.
paspalum staggers A MYCOTOXICOSIS which affects mainly cattle but also sheep and horses; it is caused by the ingestion
of tremorgenic toxins (paspalinines) when grazing Paspalum
grasses ergotized by Claviceps paspali. Symptoms: hypersensitivity to noise and movement, followed by muscle tremors
and incoordination. Recovery is usually rapid following removal
from affected pastures.
Paspalum striate mosaic virus See GEMINIVIRUSES.
passage See SERIAL PASSAGE.
passive agglutination (serol.) Any form of AGGLUTINATION in
which the combination of antibodies with antigens is made
readily detectable by the prior adsorption of the antigen or
antibody to an unrelated particulate entity e.g. a cell or a
colloidal particle. Thus, e.g., a soluble antibody or antigen may
be adsorbed to bentonite or latex (see LATEX PARTICLE TEST)
or to erythrocytes (see BOYDEN PROCEDURE); antibodies may be
adsorbed e.g. to staphylococci (see SENSITIZATION (sense 5) and
PROTEIN A). (If erythrocytes are used, the procedure is referred
to as passive haemagglutination.)
passive agglutination test Any test, involving PASSIVE AGGLUTINATION, used for detecting or quantifying specific antibodies
or antigens e.g., antibodies homologous to soluble antigens,
or particulate antigens homologous to particle-bound antibodies;
in such tests the combination of particle-bound antigen (or antibody) with homologous antibody (or antigen) causes AGGLUTINATION of the particles. Passive agglutination tests are appreciably
more sensitive than PRECIPITIN TESTS.
passive haemagglutination See PASSIVE AGGLUTINATION.
passive haemolysis See HAEMOLYSIS.
passive immunity (adoptive immunity) Temporary immunity
brought about by the transfer of pre-formed antibody, or specifically sensitized lymphocytes, from an immune individual to
a non-immune individual the latter thus becoming immune
without necessarily having had contact with the corresponding
antigen(s). Passive immunity can be acquired e.g. by transfer of
antibody via the placenta, in COLOSTRUM, or by passive IMMUNIZATION.
passive immunization See IMMUNIZATION.
Pasteur effect In organisms capable of both fermentative and respiratory modes of metabolism (e.g. Saccharomyces cerevisiae):
the inhibition of glycolysis in the presence of O2 , manifested
by the inhibition of ethanol formation and a decrease in the
amount of glucose used. This effect reflects the higher energy
yield obtained from glucose by RESPIRATION than by FERMENTATION. The Pasteur effect can apparently be explained, at least
in part, by the allosteric modulation of phosphofructokinase
DENMEYERHOFPARNAS PATHWAY).
555
Pasteurellaceae
causes disease in the absence of the microbe itself would not be
regarded as a pathogen. Thus, a toxinogenic strain of Gonyaulax
may indirectly cause paralytic SHELLFISH POISONING in man,
but it is not regarded as a human pathogen since it has never
been known to cause disease by infecting man. Similarly,
while Claviceps purpurea can be regarded as a pathogen of
certain cereals, it cannot be called a human pathogen even
though the ergot alkaloids it produces can cause ERGOTISM in
man. By analogy, Clostridium botulinum (often described as a
pathogen in medical circles) is not acting as a pathogen when
its toxin, in the absence of the bacterium, causes BOTULISM in an
adult human, although it does act as a pathogen sensu stricto
when it causes infant botulism, wound botulism, or certain
(apparently atypical) C. botulinum infections in adults. (See also
OPPORTUNIST PATHOGEN.)
By custom, disease-causing higher organisms, such as trematode worms, are referred to as parasites rather than pathogens.
(See also PARASITOLOGY.)
pathogenesis The process or mechanism of disease development.
pathogenesis-related proteins (plant pathol.) A group of lowMWt, low-IEP proteins, resistant to proteases, formed de novo
in plant tissues in response to infection with a pathogen; of
unknown function, they are thought to have a role in resistance
to disease. They were first found in tobacco cultivars exhibiting
HYPERSENSITIVITY to tobacco mosaic virus infection, but occur
in other plants infected with viruses, viroids, fungi or bacteria.
(cf. PHYTOALEXINS.)
pathogenic Able to behave as a PATHOGEN.
pathogenicity island (PAI) In a bacterial pathogen: a cluster or
cassette of genes encoding a set of virulence factors; such
sequences usually occur in the chromosome but their GC% is
typically unlike that of the chromosome suggesting acquisition
by horizontal transfer. Many PAIs (e.g. cag in Helicobacter
pylori ) are flanked by direct repeats. (cf. AVIRULENCE GENE.) A
PAI is often located at a site adjacent to a tRNA gene.
The LEE (locus of enterocyte effacement) PAI is found in all
strains of EPEC and in many strains of EHEC. LEE is a 35.5 kb
chromosomal sequence which is not flanked by direct repeats;
in EPEC it is located 16 bp downstream of the selC gene
(which encodes the tRNA for selenocysteine) [PNAS (1995)
92 16641668]. The LEE PAI encodes components of a type
III secretory system (see PROTEIN SECRETION) as well as various
effector molecules. [Type III secretory systems and pathogenicity
islands (review): JMM (2001) 50 116126.] Specific genes (and
products) include:
eae an adhesin (intimin).
espA a cellcell linking structure (?)
espB an activator of epithelial cell enzymes (?)
escN an ATPase for the secretory system (?)
tir (espE in EHEC) Tir protein (see EPEC).
(The names of genes encoding components of the type III system
in EPEC differ from those in the earlier literature; these genes
are now designated esc e.g. escN was formerly sepB.)
At least some genes in LEE (including eae, and those of
secreted proteins, such as espB ) are under transcriptional control
from a regulatory region (per ) in a plasmid (EPEC adherence
factor plasmid; EAF plasmid) found in all strains of EPEC. This
plasmid also encodes the so-called bundle-forming pili (BFP)
which may be involved in the formation of microcolonies on
the intestinal epithelium (see EPEC).
[Model of EPEC pathogenesis: TIM (1998) 6 169172.]
Other PAIs include cag in Helicobacter pylori [PNAS (1996)
93 1464814653; Nature (1997) 388 539547], and the island
PCR
PCBs Polychlorinated biphenyls (see BIOREMEDIATION).
PCC Pasteur Culture Collection.
pCF-10 See SURFACE EXCLUSION.
PCNB See QUINTOZENE.
pcnB gene See MRNA (a) and PLASMID (replication).
PCP See BIOREMEDIATION.
PCR (polymerase chain reaction) A method for copying (amplifying) specific sequences of nucleotides (see AMPLICON senses
1 and 2) in DNA; a modified form of the process (REVERSE
TRANSCRIPTASE PCR) is used for copying sequences in RNA.
PCR depends on the ability of a (thermostable) DNA polymerase to extend a primer on a template containing the amplicon
(see figure). (Patents covering PCR are owned by HoffmannLa Roche.) Other methods for amplifying nucleic acids include
LCR, NASBA and SDA; unlike PCR, the latter two methods are
conducted isothermally.
Repeated rounds of replication (i.e. ongoing cycling) in PCR
can yield millions of amplicons within hours; usually, the
sequence being copied is less than 2000 base-pairs in length,
but longer sequences have been copied.
In the basic form of PCR the reaction mixture includes: (i)
the sample (dsDNA); (ii) the primers: oligonucleotides (2030
base-pairs in length) of two types one type complementary
to the 30 end of the amplicon in one strand, the other type
complementary to the 30 end of the amplicon in the other strand;
(iii) deoxyribonucleoside triphosphates of all four types; (iv) a
thermostable DNA polymerase e.g. the Taq DNA polymerase
(see DNA POLYMERASE for examples of polymerases used in PCR).
Temperature cycling (see figure) can be controlled manually;
however, it is usually achieved by carrying out the reaction
in an instrument (a thermal cycler or thermocycler ) in which
timing is controlled automatically (see THERMOCYCLER). In most
cases, each cycle of PCR involves a sequence of three levels of
temperature: (i) e.g. 94/95 C for strand separation (denaturation
of the sample duplex DNA); (ii) a temperature suitable for the
binding of primers (annealing); and (iii) a temperature suitable
for extension, i.e. ongoing synthesis of a DNA strand, from the
primer, on the template strand. In some cases a two-temperature
protocol has been used e.g. a denaturing temperature of 94 C
and combined annealing/extension at 68 C; this is possible e.g.
with the GeneAmp 9700 system (Perkin-Elmer) amplifying a
500-nucleotide amplicon of phage l DNA.
While denaturation and extension temperatures are generally
94/95 C and 72 C, respectively, the temperature used for
annealing varies widely according to the particular assay. One
factor which influences annealing temperature is the GC% of
the primers GC%-rich primers requiring a higher annealing
temperature to avoid the formation of spurious products through
mispriming (binding of primers to inappropriate sequences in
the template). (Examples of some primer-binding temperatures:
GC% 33: 45 C [JCM (1999) 37 772774]; GC% 62: 63 C
[NAR (1998) 26 36143615].) One way of finding an optimal
annealing temperature is TOUCHDOWN PCR.
For some purposes (e.g. ARBITRARILY PRIMED PCR) a primer
is required to bind to a target sequence to which it is not
fully complementary. In such cases, PCR can be run under
so-called low-stringency conditions, i.e. particular values of
temperature, pH and electrolyte concentration which optimize
primertarget binding by helping to overcome, or minimize,
the effects of mismatches between primer and target. Highstringency conditions are those which allow primertarget
binding to occur only when the primer and target sequences
are exactly complementary, or very nearly so. The greater the
PCR
amplicon
(a)
5
(b)
(c)
PCR
was satisfactory when targets were present at the limit of the
tests sensitivity [JCM (1998) 36 191197].
Even when known inhibitors have been taken into account it
is mandatory to include suitable controls to detect the effects of
unknown/unexpected inhibitors (which may occur in only certain
batches of a given type of specimen).
Amplification facilitators are agents which can enhance the
efficiency of PCR in the presence of inhibitory substance(s);
such agents may also e.g. improve the specificity of PCR and
increase the fidelity of DNA synthesis. Amplification facilitators
include e.g. bovine serum albumin (BSA) and betaine; some
facilitators are effective against a range of inhibitors while others
have more selective activity. [Effects of amplification facilitators
on diagnostic PCR in the presence of blood, faeces and meat:
JCM (2000) 38 44634470.]
Detection of PCR products. In the standard form of PCR
the products consist of millions of amplicons whose precise
length (exact number of base pairs) is determined by the targetbinding sites of the primer pair (see figure). Such products,
all the same size, can be readily detected/identified by gel
electrophoresis as a single band at a precise location in the
gel. Typically, electrophoresis is carried out in an agarose gel,
and the band of products is detected by staining with ethidium
bromide and examining the gel under ultraviolet radiation. To
facilitate identification, another lane in the same gel is used for
electrophoresis of a set of fragments of known size (e.g. 100,
200, 300. . . base pairs); this gives a scale (ladder) with which
the experimental band(s) can be compared.
Gel electrophoresis is also used for detecting the products
in MULTIPLEX PCR (in which products of more than one size
are formed) and in ARBITRARILY PRIMED PCR (in which there are
products of very many sizes the multiple bands of products
forming a fingerprint of the sample DNA).
Band(s) of products within a gel strip may be further examined
by Southern blotting followed by SOUTHERN HYBRIDIZATION.
The identity of amplicons from a given reaction can also
be checked by subjecting them to a particular RESTRICTION
ENDONUCLEASE and checking (by electrophoresis) to see whether
fragments of expected sizes have been formed.
Amplicons can be rapidly detected by a plate-based hybridization assay. First, single-stranded amplicons are prepared by denaturing the products. These amplicons are then exposed to detector probes which are complementary to a given sequence in the
amplicon; each PROBE is labelled with the enzyme alkaline phosphatase. The whole is then transferred to a microtitre plate whose
wells have been coated with capture probes probes complementary to a different sequence in the amplicon. Incubation at
37 C permits amplicons (if present) to bind to the (surfacebound) capture probes. After washing (to remove unbound detector probes), a substrate for alkaline phosphatase is added to
detect any bound, enzyme-labelled amplicons; if present, the
enzyme will cleave the substrate, and this can be detected by
monitoring the optical density of the mixture. This method has
been used for detecting Bordetella pertussis in clinical specimens (by detecting a sequence of nucleotides specific to the
pathogen) [JCM (1997) 35 117120].
Products can also be detected rapidly by PCR DIG-ELISA.
In this method, the PCR reaction mixture includes DIGOXIGENINtagged deoxyuridine triphosphate (dUTP) so that dUMP is
incorporated into the products. Moreover, the primers are 50 biotinylated so that, after cycling, products can be captured
on the STREPTAVIDIN-coated surface of a well in a microtitre
plate. Any products captured on the wells surface can then
PCR DIG-ELISA
In microbiology, PCR is used e.g. for detecting and identifying specific microorganisms in medical or environmental specimens; this use depends on the amplification and examination of
sequences of nucleotides which are specific to the organisms of
interest. Such an approach is particularly useful for those organisms which cannot be cultured or which grow very slowly (e.g.
Mycobacterium tuberculosis). For diagnostic purposes, primers
must be specific to sequences found only in a given pathogen
(for example, a sequence in a gene encoding a unique toxin).
Examples of the use of PCR for detecting pathogens include:
Bacteroides forsythus [JCM (1999) 37 16211624], Bordetella pertussis [JCM (1999) 37 606610], chlamydiae [JCM
(1999) 37 575580], Escherichia coli O157 [JCM (1998) 36
18011804], Fusarium spp [JCM (1999) 37 24342438], group
A streptococci [JCM (1998) 36 17691771], HIV-1, HIV-2,
HTLV-I, HTLV-II [PNAS (1999) 96 63946399], rhinoviruses
[JCM (1999) 37 524530] and Trichomonas vaginalis [JCM
(1997) 35 132138].
For PCR in TYPING see: AFLP FINGERPRINTING, ARBITRARILY
PRIMED PCR, PCR-RIBOTYPING, REP-PCR, RFLP, SPOLIGOTYPING and
SSCP.
PCR is also used e.g. for (i) detecting specific virulence
factors such as toxins (e.g. diphtheria toxin) [JCM (1997)
35 16511655]; (ii) detecting genes that confer resistance to
antibiotics (e.g. the mecA gene in staphylococci [JCM (1999)
37 30293030]); (iii) surveying the diversity of species in
environmental samples by means of BROAD-RANGE PRIMERS; (iv)
DIFFERENTIAL DISPLAY.
(See also ARBITRARILY PRIMED PCR; ASYMMETRIC PCR; HOTSTART PCR; MULTIPLEX PCR; NESTED PCR; REP-PCR; REVERSE TRANSCRIPTASE PCR.)
[PCR in clinical microbiology: Book ref. 221, pp 56125.]
PCR DIG-ELISA See PCR.
PCR-ISH See IN SITU PCR.
PCR-RFLP See RFLP.
PCR-ribotyping An alternative to RIBOTYPING (q.v.) in which,
initially, PCR is used to amplify a particular sequence in the rrn
operon (usually the intergenic spacer region between the 16S and
23S genes); in many bacteria the chromosome contains multiple
copies of this sequence and, moreover, the length of the sequence
may vary even within the same chromosome. The amplicons
are examined by gel electrophoresis, giving a fingerprint of the
strain under test. Strains are classified into PCR ribotypes on
the basis of differences in their fingerprints. PCR-ribotyping
has been used e.g. for typing strains of Burkholderia [JCM
(1992) 30 20842087] and Clostridium difficile [RMM (1997)
8 (supplement 1) S55S56], and detecting species of Rhizobium
[LAM (1999) 28 137141].
PCR-SSCP See SSCP.
PDGF Platelet-derived growth factor.
pea early-browning virus See TOBRAVIRUSES.
pea enation mosaic virus (PEMV) An ssRNA-containing PLANT
VIRUS which has a narrow host range; transmission occurs
(circulatively) via aphids (e.g. Acyrthrosiphon pisi ). Virion:
icosahedral, ca. 28 nm diam.; two types occur, differing in S20
w.
Genome: two molecules of linear positive-sense ssRNA (MWts
6
ca. 1.7 and 1.3 10 ), sometimes with a third molecule of
MWt ca. 0.3 106 . PEMV replicates in the nucleus; vesicular
cytopathological structures arise from the nuclear membrane.
pea leaf roll virus See LUTEOVIRUSES.
pea mosaic virus See POTYVIRUSES.
pea streak virus See CARLAVIRUSES.
peach leaf curl See TAPHRINA.
Pediococcus
boiling water (with or without EDTA) or dilute acid (cf.
HEMICELLULOSES); they generally include PECTINS, pectic acid
and its salts (pectates), and certain neutral polysaccharides (e.g.
arabinogalactans) which occur in association with pectins.
pectic substances Syn. PECTIC POLYSACCHARIDES.
pectin See PECTINS.
pectin methylesterase See PECTIC ENZYMES.
pectinases See PECTIC ENZYMES.
pectinate (1) (adj.) Arranged like the teeth of a comb. (2) (noun)
A salt of PECTINIC ACID.
Pectinatus
A genus of Gram-negative bacteria (family BACTEROIDACEAE) which have been isolated from spoilt beers.
Cells: round-ended, slightly curved or helical rods or filaments,
0.70.8 2.032.0 m; lateral flagella arise in a line along the
concave side of the cell. Acid is formed from the fermentation
of e.g. arabinose, fructose, glucose, glycerol, lactate, maltose
and mannitol; lactate fermentation yields acetic, propionic and
succinic acids, and CO2 , as major products. GC%: ca. 40. Type
species: P. cerevisiiphilus.
pectinella One of the circumferential bands of cilia which
encircle some ciliates (e.g. Didinium). (cf. TROCHAL BAND.)
pectinesterases See PECTIC ENZYMES.
pectinic acid An outmoded term for colloidal galacturonans
which have a methyl ester content intermediate between that
of PECTINS and pectic acids.
pectinolytic (pectolytic) Able to degrade PECTINS see PECTIC
ENZYMES.
pectins The major component of the PECTIC POLYSACCHARIDES.
Pectins consist essentially of (1 ! 4)-a-D-linked galacturonic
acid residues (D pectic acid); a variable number of the C-6
carboxyl groups are methyl-esterified, and, commonly, a-Lrhamnose residues occur at intervals within the chain (forming
a rhamnogalacturonan). Other neutral sugars (e.g. L-arabinose,
D-galactose) may occur in (usually short) side-chains. Pectins
occur in the primary cell walls and intercellular regions of plants
(many fruits have a high pectin content); they also occur in the
cell walls of certain algae.
Pectins are powerful gelling agents and are widely used in
the food industry (e.g. as a setting agent in jams) and in pharmaceuticals and cosmetics. Pectin-degrading enzymes (PECTIC
ENZYMES) are produced by a wide range of microorganisms but
not by higher animals or by man. (See also RUMEN.)
Pectobacterium See ERWINIA (Carotovora group).
pectolytic Syn. PECTINOLYTIC.
Pediastrum A genus of freshwater colonial green algae (division
CHLOROPHYTA). Each colony is flat and disc-like (up to ca.
100 m diam.) and is typically made up of a central cell
surrounded by concentric rings of cells; the outermost cells each
have two lobes projecting radially outwards, so that the colony
resembles a miniature gear-wheel.
pedicel A small stalk. In the fruiting bodies of some myxobacteria: a branch of the common (main) stalk bearing a single
sporangium.
Pedinomonas See MICROMONADOPHYCEAE.
pediocin PA-1 A 44-amino-acid, pore-forming BACTERIOCIN produced by species of Pediococcus; it is active against Listeria
spp.
Pediococcus
A genus of Gram-positive bacteria of the family Streptococcaceae. Cells: non-motile cocci (ca. 1 m diam.),
commonly in pairs and tetrads. Certain vitamins and amino
acids are essential for growth. Growth occurs optimally under
microaerobic conditions; glucose is fermented homofermentatively and anaerogenically to DL-lactic acid, L(C)-lactic acid
generally predominating. (See also LACTIC ACID FERMENTATION.)
pedology
and is separated from it by an electron-translucent layer ca.
1520 nm thick. In the apicomplexan Gregarina garnhami the
three-membrane-thick pellicle forms a series of longitudinal
folds, the crests of which are associated with two sets of longitudinal filaments which have been postulated to have a role in
gliding motility [JUR (1984) 88 6676].
The typical ciliate pellicle consists of three layers of unit-type
membrane, the outermost of which (the plasmalemma) covers
the entire organism, including the cilia. The two inner layers
are sometimes called alveolar membranes; the space between
these membranes is partitioned, forming a number of vesicles
or alveoli which lie beneath the plasmalemma. Adjacent alveoli
may or may not be in communication; in some species (see e.g.
COLEPS) the alveoli contain inorganic deposits and constitute a
semi-rigid endoskeleton. The alveolar pellicle does not cover the
entire organism, and in some ciliates it forms only a relatively
small part of the cell envelope. Even when the alveolar pellicle
forms the major part of the cell envelope it is absent in the
region of the CYTOSTOME, and it is characteristically penetrated
by the MUCOCYSTS and by the kinetosomes of the cilia which
penetrate below the level of the innermost membrane. The inner
surface of the innermost membrane may be in contact with
a dense fibrillar layer of peripheral cytoplasm (the epiplasm);
the epiplasm may be the site of connection and/or anchorage
of subpellicular structures and/or pellicular structures. Some
authors consider the epiplasm to be part of the pellicle.
(See also CORTEX; KINETY; SILVER LINE SYSTEM.)
pellis (cutis; cuticle) (mycol.) Non-velar cortical layers of a
basidiocarp.
pellucid Transparent or translucent.
Pelobacter
A genus of Gram-negative, rod-shaped anaerobic
bacteria. Metabolism: fermentative; sugars are not utilized.
Species include P. acidigallici ; P. venetianus [name validation:
IJSB (1984) 34 9192]; P. carbinolicus and P. propionicus
[name validation: IJSB (1984) 34 355357].
Pelobiontida An order of naked, typically multinucleate amoebae (class LOBOSEA) which, when in motion, are typically
cylindrical or elongate-ovoid, and which lack mitochondria but
contain endosymbiotic bacteria. Flagellate stages are unknown.
The organisms are free-living in freshwater (typically microaerobic) habitats, feeding mostly on non-motile or slow-moving
algae (e.g. diatoms). The order includes the genus Pelomyxa.
(See also PSEUDOPODIUM and UROID.)
Pelochromatium roseo-viride See CHLOROCHROMATIUM AGGREGATUM.
Pelodictyon A genus of photosynthetic bacteria (family CHLOROBIACEAE). The cells are rod-like or coccoid and contain GAS
VACUOLES. Cell division occurs predominantly by binary fission;
cells of P. clathratiforme form chains which, owing to the occurrence of ternary fission in some cells in the chains, develop into
colonial structures consisting of three-dimensional networks.
Pelodinium See ODONTOSTOMATIDA.
Pelomyxa See PELOBIONTIDA.
Pelosigma
A proposed genus of filamentous bacteria which
occur, in S-shaped bundles, on mud and in fresh and brackish
waters. [Book ref. 22, p. 138.]
pelotons Coils or balls of fungal hyphae within root cortical cells
in certain endomycorrhizas.
Peltier system (thermocyclers) See THERMOCYCLER.
Peltigera
A genus of foliose LICHENS (order PELTIGERALES).
Photobiont: Coccomyxa (e.g. in P. aphthosa) or Nostoc (e.g.
in P. canina); Coccomyxa-containing species commonly have
Nostoc-containing cephalodia (see CEPHALODIUM). Thallus: typically large and more or less deeply lobed, lobes ca. 110 cm or
The nomenclature of the species of Pediococcus is confused [for discussion see Book ref. 143, pp. 179211]. Some
authors have recognized the following species as validly published: P. acidilactici, P. damnosus (formerly P. cerevisiae),
P. dextrinicus, P. halophilus, P. parvulus and P. pentosaceus.
(See also BEER SPOILAGE; IDLI; LACTIC ACID BACTERIA; MALOLACTIC FERMENTATION; MISO; PICKLING; SOY SAUCE.)
pedology Soil science.
Pedomicrobium
A genus of budding PROSTHECATE BACTERIA
found e.g. in soils; the life cycle is similar to that of HYPHOMICROBIUM but differs e.g. in that the mother cell may have many
prosthecae and typically bears a coating of iron and/or manganese compounds.
peduncle disease See COLD WATER DISEASE.
PEF PULSED ELECTRIC FIELD.
pefloxacin See QUINOLONE ANTIBIOTICS.
PEG POLYETHYLENE GLYCOL.
pegylated Refers to the form of a given molecule, prepared in
vitro, which consists of a construct containing a polyethylene
glycol moiety.
peitschengeissel flagellum See FLAGELLUM (b).
Pekilo process See SINGLE-CELL PROTEIN.
Pekin duck hepatitis B virus Syn. DUCK HEPATITIS B VIRUS.
pelagic May refer to that region of an aquatic habitat (e.g. lake,
sea) comprising the entire body of water but excluding the
BENTHIC zone, or may refer to organisms living in that region.
(See also NEKTON; NEUSTON; PLANKTON.)
Pelagophycus See PHAEOPHYTA.
Pelargonium blackleg See BLACKLEG (2).
pellet (1) The packed sedimented material formed by CENTRIFUGATION. (2) A spherical colony formed by the growth of a
mycelial fungus within a liquid medium.
pellicle (1) (bacteriol., mycol.) A continuous or fragmentary
film, or a mat of organisms, formed at the surface of a liquid
culture by certain bacteria or fungi.
A bacterial pellicle may comprise bacterial cells, extracellular
products, or both. Strains of Acetobacter xylinum (see ACETOBACTER) form a tough pellicle of CELLULOSE; each cell produces a
single cellulose ribbon composed of a number of microfibrils
which apparently emanate from distinct sites along the outer
membrane [Book ref. 38, pp. 526528]. The cellulose ribbons
from many cells aggregate to form a network which floats to the
surface of the medium, carrying the cells with it presumably
a mechanism for maintaining the organisms in the upper, oxygenated regions of the medium.
Among fungi, pellicles are formed on liquid cultures e.g. by
various yeasts (see e.g. flor yeasts in WINE-MAKING) and by
some mycelial fungi (e.g. Penicillium spp).
(2) (mycol.) Any superficial membranous structure which can
easily be removed from the tissues beneath it.
(3) (protozool.) A composite membranous structure which
forms the limiting envelope in many protozoa. In some flagellates (e.g. Trypanosoma) the pellicle consists essentially of
the cytoplasmic membrane (D plasmalemma) supported from
beneath by a system of microtubules; some authors do not
regard such a simple type of cell envelope as a pellicle. (cf.
EUGLENOID FLAGELLATES.) In coccidia (phylum APICOMPLEXA) the
pellicle of the sporozoite and merozoite stages consists of three
unit-type membranes, the outermost membrane (plasmalemma)
enclosing the entire cell; the middle and inner membranes are
closely apposed and together form the inner pellicular complex a structure which underlies the plasmalemma (except at
the MICROPORES and at regions delimited by the POLAR RINGS)
562
penicillins
more in length; only the upper surface has a cortex, the lower
surface often being tomentose and marked with veins. Conspicuous rhizines are present on the lower surface in many species.
Apothecia are formed on the upper surface often borne on narrow, erect, stalk-like extensions of the thallus margin. Species
occur e.g. on soil, rotting logs etc; many are widely distributed.
Peltigerales An order of fungi of the ASCOMYCOTINA; members include foliose LICHENS (photobiont green or cyanobacterial) which often have cephalodia. Ascocarp: APOTHECIOID, with
filiform paraphyses not forming a distinct epithecium. Asci:
bitunicate, cylindrical. Ascospores are often elongated and multiseptate. Genera: e.g. LOBARIA, NEPHROMA, PELTIGERA, PSEUDOCYPHELLARIA, SOLORINA, STICTA.
peltigeroside b-D-Galactofuranosyl-(1 ! 3)-D-mannitol, found
in Peltigera spp.
Pelvetia See PHAEOPHYTA.
pemphigus neonatorum See SCALDED SKIN SYNDROME.
penams Compounds which contain the penicillin nucleus (see
b-LACTAM ANTIBIOTICS). (cf. PENEMS.)
penciclovir A guanine nucleoside analogue ANTIVIRAL AGENT; it
is effective against alphaherpesviruses. Penciclovir is used e.g.
as a topical agent (1% in creams) for the treatment of labial and
genital herpes simplex infections. (See also FAMCICLOVIR.)
penems A class of antibiotics; a penem contains a penicillin-like
nucleus in which a double bond occurs between C-2 and C-3
(see b-LACTAM ANTIBIOTICS, Figure (a)).
penicillic acid A secondary metabolite of certain Penicillium and
Aspergillus spp; it is carcinogenic in rats when administered by
subcutaneous injection.
penicillin Any of the PENICILLINS, or (specifically) penicillin G.
penicillin acylase Syn. PENICILLIN AMIDASE.
penicillin amidase (penicillin acylase; penicillin amidohydrolase)
An enzyme (EC 3.5.1.11) produced by many Gram-positive and
Gram-negative bacteria; it cleaves the side-chain of PENICILLINS
to form 6-aminopenicillanic acid.
penicillin amidohydrolase Syn. PENICILLIN AMIDASE.
penicillin-binding proteins (PBPs) Proteins which occur in the
cell envelope of Gram-positive and Gram-negative bacteria and
which bind covalently to PENICILLINS and to related b-LACTAM
ANTIBIOTICS; according to species, there may be up to eight
distinct types of PBP in a given cell. Different PBPs vary in
their ability to bind particular b-lactam antibiotics.
The PBPs of a given species are numbered in order of
decreasing MWt (PBP-1, PBP-2 etc.); similar patterns of PBPs
occur in taxonomically related species.
PBPs have enzymic roles in the biosynthesis of PEPTIDOGLYCAN; they are thus involved e.g. in cell elongation and septum
formation. (See also CELL CYCLE and THREE-FOR-ONE MODEL.)
Some PBPs are essential for cell viability, and these constitute
the killing sites of the b-lactam antibiotics; a b-lactam antibiotic
acylates (thus inactivating) a catalytic site on a PBP.
Low-MWt (4000050000) PBPs are typically efficient
carboxypeptidases (see PROTEASES) and/or endopeptidases. In
vivo they appear to play a subordinate role, and are apparently
non-essential for cell viability.
High-MWt (>60000) PBPs are less abundant in the cell
but at least one type appears to be essential for cell viability;
they are generally more sensitive than the low-MWt PBPs to
penicillins. The enzymic roles of these PBPs include mediation
in transglycosylation and transpeptidation, i.e. the assembly
of glycan subunits and the formation of peptide cross-links,
respectively.
In Escherichia coli the high-MWt PBPs are PBP-1A, PBP-1B,
PBP-2 and PBP-3 (see below).
penicilliosis
AMOXYCILLIN, APALCILLIN, azlocillin, becampicillin, mezlocillin,
pivampicillin, and talampicillin), and by carbenicillin (6-(acarboxybenzamido)penicillanic acid) and its derivatives (e.g.
carfecillin and ticarcillin); typically, these penicillins are less
effective than benzylpenicillin against Gram-positive species.
Penicillins for oral administration (which must be acidstable) include ampicillin, phenoxymethylpenicillin and phenoxyethylpenicillin; benzylpenicillin, carbenicillin and methicillin are administered parenterally. Infrequently, penicillins can
act as ALLERGENS, the various penicillins commonly exhibiting
cross-allergenicity (cf. CEPHALOSPORINS). (See also MECILLINAM.)
[Clinical pharmacology and therapeutic uses of penicillins
(review): Drugs (1993) 45 866894.]
penicilliosis A disease of man or animals caused by a species of
Penicillium. For example, P. marneffei can cause a progressive,
disseminated, fatal human disease characterized by proliferation
of yeast-like fungal cells within histiocytes, followed by the
development of foci of necrosis and eventually abscess formation
[AJCP (1985) 84 323327].
Penicillium A genus of fungi of the class HYPHOMYCETES; teleomorphs occur e.g. in the genus TALAROMYCES. The organisms
are widespread in nature and are characteristically saprotrophic;
however, P. marneffei can cause PENICILLIOSIS (see also SUBEROSIS), and many species form toxins (see e.g. CHLOROPEPTIDE,
CITREOVIRIDIN, CYCLOPIAZONIC ACID, ERGOCHROMES, FUMITREMORGIN, GLIOTOXIN, OCHRATOXINS, PATULIN, PENITREMS, RUBRATOXINS,
VERRUCOLOGEN). Some species can cause spoilage of various
types of material (see e.g. BREAD SPOILAGE, CHEESE SPOILAGE,
PAPER SPOILAGE), some are used in manufacturing processes (see
e.g. CHEESE MAKING), and some produce useful antibiotics (see
e.g. GRISEOFULVIN, MYCOPHENOLIC ACID, PENICILLINS).
Penicillium spp form a well-developed septate mycelium; in
most species the aerial mycelium is colourless, but mycelium
within the substratum may exhibit distinctive colours the
underside (reverse) of a colony often being some shade of
yellow, orange, red or purple; diffusible pigments are formed
by some species. The conidiophores each consist essentially of
an erect or prostrate hypha (stipe), often ca. 100250 m in
length, which may be unbranched or branched. The tip of an
unbranched conidiophore may terminate in a cluster of phialides
(see CONIDIUM) (as in e.g. P. frequentans) or in a cluster of
metulae (see METULA) (as in e.g. P. variabile). In branched
conidiophores, each branch (ramus) terminates in one or more
metulae. (The term ramus is generally reserved for any cell or
hypha which occurs between a metula and its stipe; however,
confusingly, the terms ramus and metula are sometimes
used as though they were synonymous.) The terminal region
of a conidiophore (including phialides, metulae and/or rami) is
termed the penicillus. In most species the conidiophores occur as
discrete structures, but in e.g. P. claviforme and P. concentricum
they form synnemata, and in e.g. P. expansum they form
coremia. The conidia are spherical to ellipsoidal, aseptate, up to
ca. 5 m; in masses, they may be e.g. blue-green, grey-green or
yellow, according to species. Colonies may appear e.g. velvety or
woolly, and in some species they typically bear surface drops of
exudate. Sclerotia are formed e.g. by P. raistrickii and P. thomii.
Species include e.g. P. brevicompactum, P. charlesii, P. chrysogenum, P. citreoviride, P. digitatum, P. frequentans, P. griseofulvum, P. islandicum, P. italicum, P. janthinellum, P. marneffei,
P. oxalicum, P. roqueforti, and P. rubrum.
[Identification manual and atlas of Penicillium spp: Book
ref. 185.]
Penicillium brevicompactum virus See MYCOVIRUS.
peptidoglycan
In many other Gram-negative bacteria the PG is more
or less similar to that of E. coli, but many variations in
PG structure occur among the Gram-positive bacteria; for
example, backbone chains in Mycobacterium spp contain Nglycollylmuramic acid, and in Staphylococcus aureus 3050%
of the muramic acid residues are not acetylated. Even in strains
of Neisseria gonorrhoeae, though, the PG is extensively Oacetylated, and it contains 1,6-anhydromuramyl residues [JGM
(1985) 131 33973400]. The stem peptides may contain e.g.
L-lysine in place of meso-DAP (in S. aureus), and isoglutamine
instead of D-glutamic acid (in S. aureus and mycobacteria).
Cross-links between stem peptides may occur via a short
interpeptide bridge (e.g. a penta- or hexaglycine bridge in
S. aureus), and may occur in different positions in different
species. The degree of cross-linking also varies with species,
being generally more extensive in Gram-positive species. [PG
structure in staphylococci and mycobacteria: Book refs 44 and
54, respectively.]
Classification based on PG structure. The structure of PG
in a given strain tends to be constant and independent of
environmental conditions (although, exceptionally, the amino
acid content of the interpeptide bridge in staphylococcal PG can
be affected to some extent by the availability of amino acids
in the growth medium). PG structure may therefore be a useful
feature in taxonomy. Depending on the mode of cross-linking,
two basic PG types can be recognized. In group A PGs, crosslinks occur between the distal amino group of the diamino acid in
position 3 of one stem peptide and the D-alanine in position 4 of
another stem peptide; the cross-link may be direct (as in E. coli )
or may involve an interpeptide bridge (as in S. aureus). In group
B PGs an interpeptide bridge occurs between the carboxyl group
of D-glutamic acid in position 2 of one stem peptide and the
carboxyl group of D-alanine in position 4 of another. Group B
PGs are much less common than group A PGs; they are found
in certain coryneforms (e.g. strains of Agromyces, Arthrobacter,
Brevibacterium, Curtobacterium and Microbacterium), in certain
anaerobes (e.g. Acetobacterium woodii ) and in Erysipelothrix
rhusiopathiae. PG is also classified e.g. on the basis of the
nature of the peptide bridge and of the amino acid at position 3.
(See also ACTINOMYCETALES.) [Analysis of PG composition and
structure: Book ref. 138, pp 123156.]
Peptidoglycan in relation to the cell envelope. In Grampositive bacteria, PG is the major component of the cell wall and
is covalently linked to e.g. TEICHOIC ACIDS. (See also e.g. WAX
D.) The PG layer is significantly thicker than that found in most
Gram-negative bacteria. Interestingly, the thickness of the PG
layer in many cyanobacteria is similar to that typical of Grampositive species, and in at least some strains of cyanobacteria the
degree of cross-linking resembles that found in Gram-positive
bacteria [JB (2000) 182 11911199].
In Gram-negative bacteria PG occurs as a layer between the
cytoplasmic and outer membranes (see CELL WALL), and is linked
covalently to the outer membrane by the BRAUN LIPOPROTEIN.
(See also ADHESION SITE.) The content of PG may depend on
the phase of growth: e.g. in E. coli the PG is reported to
be 0.70.8% or 1.41.9% of the dry weight of log-phase or
stationary-phase cells, respectively [JB (1985) 163 208212].
It has been suggested that, in E. coli, the PG occurs as a
gel which fills the entire space between the inner and outer
membranes (periplasmic gel) [JB (1984) 160 143152]; it was
proposed that this gel may be more extensively cross-linked
near the outer membrane, becoming progressively less crosslinked towards the cytoplasmic membrane, and that periplasmic
acids via xylulose 5-phosphate and the phosphoketolase reaction (Appendix III (d and b), [AvL (1983) 49 209224]); the
pentoses are taken up either by specific permeases or by PEPdependent phosphotransferase systems (see PTS). (Thermobacteria are unable to ferment pentoses.) In e.g. Bacillus spp,
some enterobacteria and certain yeasts pentoses/pentuloses are
converted [as in Appendix III(d)] to xylulose 5-phosphate, ribulose 5-phosphate or ribose 5-phosphate which can enter the HEXOSE MONOPHOSPHATE PATHWAY [Appendix I(b)].
(See also ARA OPERON and INDUSTRIAL ALCOHOL.)
pentostatin See VIDARABINE.
pentraxin proteins See ACUTE-PHASE PROTEINS.
pentulose See PENTOSES.
PEP Phosphoenolpyruvate.
PEP-dependent phosphotransferase system See PTS.
PEP potential The sum of the intracellular concentrations of
phosphoenolpyruvate (PEP) and 2-phosphoglycerate [JB (1977)
130 583595]. In cells of e.g. streptococci, high intracellular
levels of these compounds develop during starvation, ensuring
that when sugars become available they can be taken up rapidly
by the (PEP-dependent) PTS. (See also FLUORIDES.)
peplomer See ENVELOPE (sense 1).
peplos Syn. ENVELOPE (sense 1).
pepsin A PROTEASE (EC 3.4.23.1) which is present in the stomach
in most vertebrates and which shows maximum activity at low
pH (ca. 12); it is denatured at pH >6.
pepstatin A peptide inhibitor of aspartyl proteases such as
PENICILLOPEPSIN.
peptidase Syn. PROTEASE.
peptide antibiotics See e.g. BACITRACIN, CECROPINS, DEFENSINS,
EDEINES, GRAMICIDINS, POLYMYXINS, TYROCIDINS.
peptide nucleic acid (PNA) See PNA.
peptidoglycan (murein; mucopeptide; glycosaminopeptide) A
heteropolymer which is found in the CELL WALL of most bacteria
(cf. e.g. PASTEURIA and PLANCTOMYCES), and which is also present
in the cortex of bacterial ENDOSPORES, but which is not found
in members of the ARCHAEA (cf. PSEUDOMUREIN). Peptidoglycan
(PG) is the component which is primarily responsible for the
mechanical strength of the cell wall (protecting the cell e.g.
against osmotic lysis) and for maintaining the shape of the cell.
Structure of PG. PG consists essentially of linear, heteropolysaccharide backbone chains that are cross-linked, via short
peptides, to form a net-like molecule (the murein sacculus
see (a) in the figure); in almost all cases the sacculus envelops the bacterial protoplast (incomplete, or patchy, peptidoglycan occurs e.g. in Myxococcus xanthus: see MYXOBACTERALES).
In Escherichia coli, the backbone chains consist of alternating
(1 ! 4)-b-linked residues of N-acetyl-D-glucosamine (GlcNAc)
and its 3-O-D-lactyl ether derivative, N-acetylmuramic acid
(MurNAc). A MurNAc residue may be linked, via its carboxyl
group, to a short peptide (the stem peptide) commonly the
tetrapeptide L-alanine D-glutamic acidmeso-diaminopimelic
acid D-alanine. Cross-links between the backbone chains are
formed directly between the D-alanine of one stem peptide and
the meso-diaminopimelic acid (meso-DAP) of another on an
adjacent chain (see (b) in figure). The backbone chains run perpendicular to the long axis of the cell.
Each peptide bridge shown in the figure links a given
backbone chain to one of the other backbone chains. However,
as described in the legend, some peptide bridges link together
more than two backbone chains, and such links are essential
features in the THREE-FOR-ONE MODEL of peptidoglycan growth.
565
free peptide
G
G
M
G
M
G
M
G
M
G
M
backbone
chains
cross-link
G
M
N -acetylglucosamine residue
G
(a)
N -acetylmuramic
acid residue
6
O
H
CH2OH
5
N -acetylglucosamine
residue
H
H
3
CH2OH
H
O
O
H
OH
H
O
H
H
NH
NH
lysozyme
acts here
O
CH.CH3
CO
CO.CH3
CO.CH3
CH2OH
H
NH
CO
L-ala
CH.COOH
(CH2)2
CO
D-glu
(CH2)3
CO
meso-DAP
CO.CH3
NH
CO.CH3
NH
NH
CH.CH3
CH.CH3
CO
NH2CH.COOH CO
free -amino group
available for trimer
formation
H
H
NH
CH.CH3
NH
CH.CO
H
OH
NH
CH.CH3
CH2OH
NH
CH.COOH
D-ala
(CH2)2
cr
os
CO
s-
lin
NH
CH.CO
(CH2)3
NH.CH.COOH
NH
CH.CH3
COOH
(b)
PEPTIDOGLYCAN. The structures shown are typical of those in Escherichia coli; similar types of peptidoglycan are found in many other
Gram-negative bacteria. (Continued on page 567.)
566
peptidoglycan
proteins may diffuse freely in the gel. However, this would
imply multilayered PG, and measurements of the turnover of PG
in E. coli have suggested that the lateral wall of the cell may
contain a monolayer of PG, with multilayered PG probably at
the poles of the cell [JB (1993) 175 711].
Biosynthesis of peptidoglycan in E. coli. The initial step
in biosynthesis may be regarded as the formation of the
UDP (uridine 50 -diphosphate) derivative of N-acetylglucosamine
(here designated UDP-GlcNAc); this occurs in the cytoplasm.
Some of the UDP-GlcNAc is converted to UDP-Nacetylmuramic acid (UDP-MurNAc). This conversion begins
with a reaction between UDP-GlcNAc and phosphoenolpyruvate
catalysed by the enzyme phosphoenolpyruvate:UDP-GlcNAc
enolpyruvyl transferase; the UDP-GlcNAc-3-enolpyruvyl ether
intermediate is reduced to UDP-MurNAc in an NADPHdependent reaction. (Conversion of UDP-GlcNAc to UDPMurNAc is blocked by FOSFOMYCIN.)
Still within the cytoplasm, amino acids are added sequentially to
UDP-MurNAc by enzymes that require ATP and magnesium (or
manganese) ions to form UDP-N-acetylmuramylpentapeptide
(the Park nucleotide), which includes a terminal D-alanyl-Dalanine (added as a dipeptide). (See also CYCLOSERINE.) The
Park nucleotide is then transferred, with release of UMP, to
BACTOPRENOL monophosphate in the cytoplasmic membrane.
UDP-GlcNAc is subsequently incorporated, with release of UDP,
to complete the bactoprenoldisaccharidepentapeptide subunit
(a step which is inhibited by NISIN).
Disaccharidepentapeptide subunits are transferred from the
cytoplasmic membrane to the periplasmic region. Such transfer (blocked by VANCOMYCIN) involves release of the bactoprenolpyrophosphate (bactoprenolPP) which thus remains
in the cytoplasmic membrane. BactoprenolPP must be dephosphorylated (by a membrane-bound pyrophosphatase) to the
monophosphate form before it can again act as an acceptor of
the PMurNAcpentapeptide; dephosphorylation is inhibited by
BACITRACIN.
In the periplasm, the disaccharidepentapeptide subunits are
inserted into the growing peptidoglycan sacculus. According to
one scheme [Microbiology (1996) 142 19111918], the disaccharides are polymerized (forming new backbone chains) by
transglycosylation reactions that involve the enzymic activities of PENICILLIN-BINDING PROTEINS (see also MOENOMYCIN).
(Although transglycosylation reactions seem to be catalysed
primarily by penicillin-binding proteins, a penicillin-insensitive
glycan polymerase, distinct from PBPs, has been reported in
PEPTIDOGLYCAN (continued) (a) The three-dimensional net-like peptidoglycan molecule: backbone chains of alternating residues of Nacetylglucosamine (G) and N-acetylmuramic acid (M) are held together by short peptides which link N-acetylmuramic acid residues. Each of
the peptide bridges shown in the diagram links a given backbone chain to one other backbone chain. However, there are also peptide bridges
which link together more than two backbone chains; the different types of peptide bridge in E. coli are briefly described in (b), below.
(b) Part of two adjacent backbone chains showing the mode of linkage between them. Each N-acetylmuramic acid residue bears a short
stem peptide in this example, the tetrapeptide L-alanine D-glutamic acidmeso-diaminopimelic acid(meso-DAP) D-alanine (shown in dotted
boxes); in this kind of peptide bridge there is a direct, covalent link between the D-alanine of one stem peptide and the e-amino group of
meso-DAP in the other stem peptide. As this particular type of peptide bridge involves two stem peptides, each consisting of four amino acid
residues, it has been referred to as a tetra-tetra dimer (or a tetra-tetra). Another type of peptide bridge, the tetra-tri-dimer (tetra-tri), is formed
from one tetrapeptide and one tripeptide. A trimer peptide bridge is one which links together three of the glycan backbone chains; this occurs
when a stem peptide on a third backbone chain forms a covalent linkage with the free e-amino group (see diagram) of a dimer bridge. An
appreciation of these different types of peptide bridge is essential for understanding the 3-for-1 model (THREE-FOR-ONE MODEL) of replication of
the peptidoglycan sacculus.
The enzyme lysozyme hydrolyses the N-acetylmuramyl-(1!4) linkages in the backbone chain (see diagram); such activity weakens the cell
envelope, and may lead to osmotic lysis.
Reproduced from Bacteria, 5th edition, Figure 2.7, pages 2021, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN
0471-98880-4) with permission from the publisher.
567
peptidyl transferase
anaerobia be included within the genus Peptostreptococcus as
P. tetradius [IJSB (1983) 33 683698]. (For P. elsdenii see
MEGASPHAERA.) (cf. PEPTOCOCCUS.)
per locus See PARTITION.
Per phenotype Phage-encoded resistance phenotype (see LACTIC
ACID STARTERS).
Peritrichia
perilemma In many oligotrich ciliates: a membrane external to
the pellicle.
perimycin (syn. fungimycin) A PEROSAMINE-containing heptaene
POLYENE ANTIBIOTIC produced by a strain of Streptomyces
coelicolor.
perinuclear space See NUCLEUS.
periodic acidSchiff reaction See PAS REACTION.
periodontitis An acute or chronic inflammation of toothsupporting tissues. The periodontium includes the periodontal
ligament: a cup-like mass of fibrous connective tissue which
binds the root of the tooth to the tooth socket in the jaw bone; the
term periodontium may also include the cementum (a bone-like
substance which invests the root of the tooth), the free gingiva
(see GINGIVITIS), and the alveolar bone (i.e. that part of the jaw
bone which forms the tooth socket that binds the periodontal
ligament.
Periodontitis is promoted by the accumulation of DENTAL
PLAQUE in or near the gingival sulcus: the shallow groove
(12 mm deep) at the toothgum junction; under these conditions the gum may shrink away from the tooth (the gingival
sulcus enlarging to form a periodontal pocket) thus exposing
the cementum and the periodontal ligament to microbial attack.
In periodontal disease there is an increased flow of CREVICULAR FLUID.
Various bacterial species have been causally connected with
periodontitis, but the aetiology of the disease is not yet fully
understood; the human oral microflora has not yet been fully
characterized, and it is possible that currently uncultured organisms may contribute to periodontitis. In one study, samples of
healthy and periodontic material were examined with the object
of investigating (from PCR-determined sequence data) whether
any specific types of organism correlate with disease; one organism, whose data suggested a close relationship to asaccharolytic
Eubacterium spp, was found only in deep pockets in periodontitis patients, possibly indicating an association with advanced
periodontitis [JCM (1999) 37 14691473].
Bacteria which have been aetiologically linked to periodontitis
include species of BACTEROIDES (e.g. B. gingivalis) and FUSOBACTERIUM; Actinobacillus actinomycetemcomitans and Capnocytophaga sp have been implicated in juvenile periodontitis. (See
also CENTIPEDA.)
Multiplex PCR has been used for the simultaneous detection
of Bacteroides forsythus and Prevotella intermedia in 152
clinical samples, including 38 specimens of plaque [JCM (1999)
37 16211624].
peripheral membrane cylinder See ASCUS.
peripheral membrane protein See CYTOPLASMIC MEMBRANE.
periphyses (sing. periphysis) Short, sterile filaments which form
a lining in the ostiolar canal in a perithecium or pseudoperithecium.
periphyton community Syn. AUFWUCHS.
periplasm Syn. PERIPLASMIC REGION.
periplasmic binding protein Syn. BINDING PROTEIN (sense 1).
periplasmic fibrils See SPIROCHAETALES.
periplasmic flagella See SPIROCHAETALES.
periplasmic gel See PEPTIDOGLYCAN.
periplasmic region (periplasmic space; periplasm) In Grampositive bacteria and archaeans: the region between the
CYTOPLASMIC MEMBRANE and the CELL WALL; in Gram-negative
bacteria: the region between the cytoplasmic membrane and the
OUTER MEMBRANE or, according to some authors, between the
cytoplasmic membrane and the layer of PEPTIDOGLYCAN.
Certain enzymes and other proteins are located partially or
entirely in the periplasmic region and may be released from
OSMOTIC SHOCK.
TION.)
periplasmic space Syn. PERIPLASMIC REGION.
periplast The cell envelope, or particular layer(s) of the cell
envelope, in certain algae and protozoa; see e.g. PELLICLE
(sense 3) and CHOANOFLAGELLIDA.
Peripylaria A category (section) of LEISHMANIA species which
multiply in the anterior part of the hindgut of the arthropod vector, and then migrate to the pharynx, cibarium and proboscis;
it includes e.g. L. braziliensis and L. tarentolae. (cf. HYPOPYLARIA, SUPRAPYLARIA.)
periseptal annulus In Gram-negative bacteria: a continuous
circumferential fusion between the OUTER MEMBRANE and the
cytoplasmic membrane, one annulus occurring on each side of
the site of cell division thus delimiting a small periplasmic
compartment at the site of future septum formation. [PNAS
(1983) 80 13721376.] (cf. ADHESION SITE.)
peristome (1) The buccal cavity, or the extreme distal part of the
buccal cavity, together with the somatic region adjacent to it; the
term is used primarily for the appropriate parts in peritrichs and
in certain spirotrichs, but it is sometimes used for the convoluted
distal region of some chonotrichs. (cf. INFUNDIBULUM.) (2) Syn.
BUCCAL CAVITY.
perithecioid Having the general characteristics of a PERITHECIUM.
perithecioid pseudothecium See ASCOSTROMA.
perithecium A hollow, spheroidal or flask-shaped ASCOCARP (ca.
100300 m) which opens to the exterior via an OSTIOLE; asci
develop inside the perithecium, commonly in the form of a
hymenial layer or as a basal tuft. According to species, perithecia
may develop on the surface of a substratum or fungal STROMA,
or embedded within a fungal stroma, and the wall (peridium) of
a perithecium may be membranous or brittle, brightly coloured
or dark. Some perithecia contain (in addition to asci) sterile
structures such as paraphyses. (For ascospore discharge see
ASCOSPORE.) Perithecia are formed e.g. by members of the
SORDARIALES and SPHAERIALES.
(cf. ASCOSTROMA (pseudoperithecium).)
peritonitis Localized or generalized inflammation of the peritoneum (the membrane which lines the abdominal cavity and
covers the viscera).
peritrich A member of the PERITRICHIA.
Peritrichia A subclass of freshwater, estuarine and marine ciliate
protozoa (class OLIGOHYMENOPHOREA); one order: Peritrichida.
In mature peritrichs, the somatic ciliature is limited or absent,
but the oral ciliature is well developed and includes rows of
cilia which looking into the buccal cavity spiral downwards
towards the cytostome in an anticlockwise (counterclockwise)
direction. According to species, individual cells may be shaped
like an egg, bell or bottle etc; in some species the cell (zooid ) is
attached to the substratum either directly or by means of a contractile or non-contractile stalk. Some species are loricate, and
some form colonies. STOMATOGENESIS is buccokinetal. Asexual
reproduction in sedentary species may occur e.g. by budding
with the formation of a motile, ciliated larva (telotroch).
Predominantly sedentary peritrichs are placed in the suborder Sessilina (genera: e.g. Apiosoma, Campanella, CARCHESIUM, Ellobiophrya, Epistylis, Lagenophrys, OPERCULARIA, Rhabdostyla, Scyphidia, Vaginicola, VORTICELLA, Zoothamnium).
The mobile peritrichs (all ecto- or endoparasitic, occasionally pathogenic, in freshwater or marine vertebrates and
invertebrates) are placed in the suborder Mobilina (genera: e.g.
Leiotrocha, Trichodina, Vauchomia).
569
Peritrichida
peroxidaseantiperoxidase technique See PAP TECHNIQUE.
peroxin See PEX MUTATION.
peroxynitrite See NITRIC OXIDE.
peroxisome A type of MICROBODY found in many kinds of
eukaryotic cell, including certain fungi, protozoa and algae.
Peroxisomes contain a range of enzymes including e.g. peroxidase, CATALASE, D-amino acid oxidase, dehydrogenase and acyl
transferase. Each peroxisome is typically rounded, with a granular matrix and commonly an electron-dense core (D nucleoid);
it is bounded by a single trilaminar membrane 4.58 nm
in thickness. Peroxisomes apparently develop by incorporating
their component proteins (synthesized on free polysomes) and
eventually dividing into daughter peroxisomes; this contrasts
with the earlier view of biogenesis which supposed that peroxisomes budded from the endoplasmic reticulum.
In animal-type cells, peroxisomes carry out a range of
functions which (depending on type of cell) include respiration,
oxidation of alcohol and fatty acids, synthesis of plasmalogens,
and purine metabolism; in plant/algal cells, functions include
GLUCONEOGENESIS and PHOTORESPIRATION.
In methylotrophic yeasts (see METHYLOTROPHY) the peroxisomes, which contain methanol oxidase, occur in greater number
and size when the yeasts are grown on methanol (rather than e.g.
glucose). [Peroxisomes in methylotrophic yeasts: AMP (1983)
24 182.] (See also HYDROCARBONS.)
[Recent developments in peroxisome biology: Endeavour
(1996) (new series) 20 6873.]
[Peroxisome membrane proteins (role in biogenesis and function of the peroxisome): FEMS Reviews (2000) 24 291301.]
persistence (virol.) The phenomenon in which a virus remains
within a cell, organism or population [Book ref. 90] for a
prolonged period of time, during which it may or may not
replicate to produce infectious progeny virions; if the virus
persists in cryptic form, without production of infectious virions
and without causing symptoms in the host, it is said to be
latent. (Some authors reserve the term persistence for those
cases in which infectious virions are continually produced [Book
ref. 148, p. 161].)
In a host organism, persistence (sensu lato) may be established directly or may follow an acute phase of disease. Various
categories of persistent infection can be distinguished. (a) Infectious virions are not produced and infection is asymptomatic
(latent infection); in some cases the virus may, under certain
conditions, be reactivated to produce infectious virions and
cause sporadic recurrences of illness (see e.g. HERPES ZOSTER).
(b) Infectious virions are not produced, but disease may nevertheless eventually occur (see e.g. SUBACUTE SCLEROSING PANENCEPHALITIS). (c) Infectious virions are continually produced but
no symptoms are apparent resulting in a CARRIER (sense 1).
(See also LCM VIRUS.) (d) Infectious virions are continually produced, and ongoing chronic disease results.
Viral strategies for persistence in cells/hosts include e.g.
integration of viral nucleic acid into host chromosomal DNA (as
in the RETROVIRIDAE), or maintenance of viral nucleic acid in a
stable extrachromosomal form (see e.g. EPSTEINBARR VIRUS); in
some cases impaired immunological responses or immunological
tolerance may be important factors. In cell cultures, persistence
may result from the formation of viral mutants or of DEFECTIVE
INTERFERING PARTICLES. (See also CARRIER CULTURE.)
persistent generalized lymphadenopathy See AIDS.
persistent virus (1) See CIRCULATIVE TRANSMISSION. (2) A virus
which can establish a persistent infection (see PERSISTENCE).
pertactin A cell-surface adhesin found in species of Bordetella.
petroleum
perthophyte Syn. PERTHOTROPH.
perthotroph (perthophyte) (1) A parasite which kills tissues
within a living host, subsequently deriving nutrients from the
dead tissues. (2) An organism which derives nutrients from dead
tissues within a living host whether or not it kills those tissues
itself. (The term is usually applied to plant/microorganism
interactions.) (cf. BIOTROPH; NECROTROPH.)
Pertusaria A genus of crustose LICHENS (order PERTUSARIALES);
photobiont: a green alga. Apothecia frequently occur several
together in warts on the thallus; they are initially peritheciumlike with a pore-like opening, but in some species they subsequently open out to form flat or concave discs. In P. pertusa, the
periphery of the thallus is surrounded by a white hypothallus;
the apothecia do not open out as they mature. In P. amara, the
thallus bears scattered white soralia (0.51.5 mm diam.) which
have a bitter taste due to the presence of picrolichenic acid;
apothecia are rare, but when present they are solitary and the
mature discs are open and sorediate. Species occur e.g. on bark.
Pertusariales An order of fungi of the ASCOMYCOTINA; members include crustose LICHENS (photobiont commonly green),
and saprotrophic and lichenicolus fungi. Ascocarp: APOTHECIOID, sometimes lirelliform. Asci: bitunicate. Genera: e.g.
OCHROLECHIA, PERTUSARIA.
pertussigen Syn. PERTUSSIS TOXIN.
pertussis Syn. WHOOPING COUGH.
pertussis toxin (pertussigen; islet-activating protein; histaminesensitizing factor; leucocytosis-promoting factor) An exotoxin,
produced by Bordetella pertussis, which is one of the virulence
factors associated with WHOOPING COUGH (see also CYCLOLYSIN,
DERMONECROTIC TOXIN, TRACHEAL CYTOTOXIN).
The structure of pertussis toxin (PT) resembles that of e.g.
CHOLERA TOXIN and SHIGA TOXIN: all of these toxins have an
AB5 arrangement of subunits in which five B subunits form a
pentameric ring, and the A subunit occupies a central position
to one side of the plane of the ring.
The B subunits of PT are not identical; some of them have
binding sites for specific receptor molecules on eukaryotic target
cells.
The A subunit is a 26 kDa protein with ADP-ribosyl transferase activity. Within the target cell it ADP-ribosylates a particular heterotrimeric G protein, Gi (D Ni ), which normally inhibits
the activity of ADENYLATE CYCLASE; ADP-ribosylation inhibits
Gi , leading to an increase in the intracellular concentration of
cyclic AMP (cAMP). (cf. CHOLERA TOXIN.)
B. parapertussis apparently contains a silent (i.e. nonexpressed) gene for pertussis toxin.
Pesotum See CERATOCYSTIS and HYPHOMYCETES.
Pestalotia See MELANCONIALES.
peste des petits ruminants (syn. pseudorinderpest) A disease
of sheep and goats which occurs in W. Africa. Symptoms
include fever, nasal and ocular discharge, and necrotic stomatitis,
followed by severe enteritis and pneumonia; mortality rates may
be >90%.
The causal agent is a virus (the Kata virus) of the genus
MORBILLIVIRUS.
pesticin I A BACTERIOCIN produced by strains of Yersinia
pestis; it is active against Y. pseudotuberculosis and strains of
Escherichia coli. Production of pesticin I correlates with the
production of a fibrinolytic factor and a coagulase.
pestis minor A mild form of PLAGUE in which buboes are formed
without systemic symptoms.
Pestivirus
A genus of viruses (family TOGAVIRIDAE) which
infect pigs (SWINE FEVER virus) and ruminants (BOVINE VIRUS
571
phagocytosis
of the grid is inoculated with one drop of a phage suspension
(at ROUTINE TEST DILUTION) each square being inoculated with
a different phage; the plate is then incubated. Each of the phages
used for typing is lytic for one strain, or a limited number
of strains, of the species under test; a phage which lyses the
particular strain being tested will form a clear macroscopic
area amid the opaque layer of bacterial growth. The test strain
can then be defined in terms of the phages to which it is
sensitive. (The results of phage typing may be affected if the
bacterium under test carries a PLASMID encoding a RESTRICTION
ENDONUCLEASE which destroys phage nucleic acid.) Strains of
Salmonella typhi which bear the VI ANTIGEN may be typed by a
range of phages each of which is specific for one or more of the
Vi strains of S. typhi ; this procedure is often termed Vi phage
typing.
phagemid A CLONING vector which includes (i) a plasmids
origin of replication; (ii) a multiple cloning site (MCS), i.e. a
POLYLINKER; (iii) a marker gene (e.g. a gene encoding resistance
to kanamycin); and (iv) the origin of replication of a filamentous
phage (e.g. that of the ssDNA phage f1). The DNA sample (to
be cloned) is inserted via the MCS, and the phagemid is then
inserted into a bacterium e.g. by transformation.
A phagemid can be used e.g. for making double-stranded
copies of the given fragment (i.e. used as a conventional cloning
vector). It can also be used for making single-stranded copies
if the phagemid-carrying bacteria are infected with a helper
phage, e.g. phage M13, which promotes replication from the
phage origin in the phagemid; the single-stranded copies are
packaged into phage coat proteins (encoded by the helper phage)
and exported to the medium. When freed from phage coat
proteins, the single-stranded copies of the insert can be used
e.g. for sequence analysis (see DNA SEQUENCING).
A phagemid may contain a promoter on each strand, either
side of the MCS, so that, if required, the cloned fragment can
be transcribed.
phagocyte Any cell which can carry out PHAGOCYTOSIS particularly a neutrophil or macrophage.
phagocytosis The process in which particulate matter is ingested,
and usually digested, by certain types of cell or microorganism
(cf. PINOCYTOSIS). In mammals, phagocytosis by certain leucocytes is an important aspect of the immune defence system, while
in some microorganisms phagocytosis is a mode of feeding.
(a) In mammals, phagocytosis is carried out e.g. by NEUTROPHILS
and MACROPHAGES. Essentially, the particle (e.g. an opsonized
bacterium) initially binds to the surface of the phagocyte; the
phagocytes cytoplasmic membrane then invaginates to form
a pocket which contains the particle. (Different intracellular
signals may be generated in the phagocyte according to whether
engulfment was triggered from antibody- or complement-binding
sites.) Subsequently, the invaginated membrane forms a closed,
intracellular sac or vacuole, the phagosome. (A phagosome
which contains a parasite is called a parasitophorous vacuole.)
The pH within the phagosome decreases, and the phagosome
coalesces with one or more LYSOSOMES to form a phagolysosome
(D lysophagosome) within which the bacterium etc. may be
killed and degraded.
The maturation of a phagosome into a phagolysosome can be
monitored from changes in (i) its internal pH, and (ii) the associated proteins; for example, a phagolysosome is characterized by
so-called lysosome-associated membrance proteins (LAMPs).
Antimicrobial activity within phagocytes is promoted by
(i) the wide range of lysosomal enzymes, and (ii) the intracellular formation of certain toxic derivatives of oxygen see
phagolysosome
and
(species formed during the oxidative burst
(D respiratory burst) characteristic of some types of phagocyte); such derivatives are formed e.g. by neutrophils and
macrophages. In NEUTROPHILS (q.v.), the oxygen derivatives are
generated within 3060 seconds of cell-surface stimulation. Ferric ions bound to lysosomal LACTOFERRIN may serve to promote
the formation of hydroxyl radical from hydrogen peroxide and
superoxide. During the oxidative burst, the consumption of oxygen by the phagocyte increases sharply. (See also CHEMILUMINESCENCE.) Reactive oxygen derivatives are also released to the
extracellular environment.
Some bacteria can resist ingestion by phagocytes as a consequence of their capsular or cell-wall components. For example,
the capsule of Bacillus anthracis is anti-phagocytic (cf. STERNE
STRAIN). Again, the PROTEIN A cell-wall component of Staphylococcus aureus may serve to inhibit opsonization by binding the
Fc portion of antibodies.
Some pathogens can kill phagocytes: see e.g. APOPTOSIS and
LEUCOCIDINS.
Certain pathogens (e.g. Coxiella, Leishmania spp, Listeria
monocytogenes and Mycobacterium lepraemurium) can survive or grow within phagosomes, or phagolysosomes, avoiding
destruction by various mechanisms. For example, in the case
of Chlamydia spp, Legionella pneumophila and Mycobacterium
tuberculosis the phagosome does not acidify and does not fuse
with the lysosome. Under certain circumstances, some pathogens
(e.g. Mycobacterium leprae, Rickettsia mooseri, Trypanosoma
cruzi ) can escape from the phagosome and grow within the
cytoplasm of the phagocyte. (See also REOVIRUS.)
Phagosomes containing live Toxoplasma gondii resist fusion
with lysosomes, and T. gondii may also fail to trigger the phagocytes oxidative mechanism and may inbibit development of
the normal acidification of the phagosome. M. leprae apparently fails to stimulate the generation of superoxide anion by
the phagocyte.
In some cases a pathogen is not taken up and killed because it
has actually invaded the phagocyte. Invasion may involve uptake
via adhesins and receptors which differ from those involved in
routine phagocytosis. The initial contact between pathogen and
phagocyte may be important in determining the pathogens fate;
for example, of the various modes of binding, some may favour
survival by failing to trigger an oxidative burst within the phagocyte. In the case of Legionella pneumophila, the phagosome in
a macrophage maintains near-neutral pH, and the pathogen is
able to multiply, killing the phagocyte. In this organism the icm
(intracellular multiplication) genes also called dot (defect in
organelle trafficking) genes are believed to encode a secretory system (and associated effector molecules) involved e.g. in
blocking phagosomelysosome fusion; mutations in these genes
have been found to affect the pathogens ability to multiply
within, and kill, macrophages [see e.g. TIM (1998) 6 253255].
It has been reported that the zinc metalloprotease secreted by
L. pneumophila inhibits (i) the oxidative burst, and (ii) chemotaxis in phagocytes [JMM (2001) 50 517525].
In the case of Mycobacterium tuberculosis, invasion/survival
may be influenced by (i) the cell-surface chemistry of the given
strain; (ii) the site of infection (e.g. lung); and (iii) the timing of
pathogenphagocyte contact (e.g. at initial infection, or later).
The opsonization of M. tuberculosis may occur via any of
four pathways of COMPLEMENT FIXATION (q.v.); however, nonopsonic (complement- and antibody-independent) binding of the
pathogen to the phagocyte may be important for initial infection
e.g.
HYDROXYL RADICAL
574
phase variation
of actin filaments; consequently, cellular functions associated
with the microfilament system (e.g. cytoplasmic streaming, cell
motility) are irreversibly blocked. (See also MYCETISM.)
Phallus See PHALLALES.
Phanerochaete See APHYLLOPHORALES (Corticiaceae).
phaneroplasmodium See MYXOMYCETES.
pharyngeal basket Syn. CYRTOS.
pharyngeal rod organ See PERANEMA.
pharyngitis Inflammation of the pharynx. Acute pharyngitis is
often caused by Streptococcus pyogenes; symptoms include e.g.
sore throat, fever, pharyngeal exudate. Other causes include any
of a range of viruses e.g. adenovirus (see PHARYNGOCONJUNCTIVAL FEVER), COMMON COLD viruses, coxsackieviruses (see also
HERPANGINA), EB virus (see INFECTIOUS MONONUCLEOSIS).
pharyngoconjunctival fever A (usually mild) disease, affecting mainly children and young adults, caused by certain adenoviruses (see MASTADENOVIRUS). Symptoms: fever, inflammation
of conjunctivae and/or pharynx, and enlargement of cervical
lymph nodes.
phase-contrast microscopy See MICROSCOPY (c).
phase degradation Phase variation in BORDETELLA.
phase-shift mutation Syn. FRAMESHIFT MUTATION.
phase variation Spontaneous switching from the synthesis of a
given cell-surface component to the synthesis of a different form
of that component or the starting, or stopping, of synthesis of
such a component; each form of a given component depends on
the expression of a specific allele, so that the number of different
forms of that component depends on the allelic complement of
the organism (cf. ANTIGENIC VARIATION).
The term phase variation was initially applied to the
alternation of flagellar components in Salmonella, but is now
applied more generally to a range of phenomena involving
variation in cell surface components. Many of these phenomena
are known to involve re-arrangements of DNA.
Some well-studied examples of phase variation include the
prototypical flagellar phase variation in Salmonella (see below);
the on/off switching of type I FIMBRIAE (q.v.) in Escherichia coli;
mRNA
H2
H1 repressor
H2
H1 repressor
H1
mRNA
H1
PHASE VARIATION: alternation of flagellar proteins in Salmonella (principle, diagrammatic; see entry).
In most strains of Salmonella the flagellar filament contains either of two distinct types of protein, encoded by genes H1 and H2. Normally,
only one of these genes is expressed at any given time, so that the flagellar filament contains either the H1 gene product or the H2 gene
product.
The promoter ( ) of the H2 operon is flanked by two short inverted repeats ( ) which are recognized by a site-specific recombinase; that
is, the sequence containing the promoter can be inverted by site-specific recombination.
Top. The position of the H2 promoter is such that the H2 operon can be transcribed. The H2 gene product is incorporated in the flagellar
filament, and the H1 repressor protein blocks transcription of the H1 gene.
Below. Site-specific recombination has occurred between the two inverted repeats, so that the sequence containing the H2 promoter has
been inverted. In this new orientation the H2 promoter is no longer functional. Because the H2 operon is not transcribed, the H1 repressor is
not formed, and this permits transcription of the H1 gene so that the flagellar filament now contains the H1 gene product.
Reproduced from Bacteria, 5th edition, Figure 8.3, page 168, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
575
phaseollidin
EXCLUSION.) When cultured in a fresh medium, F phenocopies
revert to the donor state.
Studies on F phenocopies reveal e.g. a low level of nicking
at oriT in the late stationary phase although the F pilus
transfer apparatus appears to be maintained in the cell envelope
even after cessation of transcription of the main transfer region
[Microbiology (1998) 144 25792587].
phenogram Any dendrogram which expresses phenetic relationships. (cf. CLADOGRAM.)
phenol (as a disinfectant) See PHENOLS.
phenol coefficient A number which expresses the antimicrobial
activity of a given phenolic DISINFECTANT relative to that of
phenol under standard conditions; it can be determined by e.g.
the RIDEALWALKER TEST or the CHICKMARTIN TEST.
phenol red A PH INDICATOR: pH 6.88.4 (yellow to red); pKa
7.9.
phenolates (in iron uptake) See SIDEROPHORES.
phenolic disinfectants See PHENOLS.
phenolphthalein A PH INDICATOR: pH 8.310.0 (colourless to
red); pKa 9.6.
phenols (as ANTISEPTICS and/or DISINFECTANTS) Phenol and its
derivatives (phenolics cresols, xylenols etc) are microbistatic
or microbicidal, depending on e.g. concentration and temperature; they may act e.g. by affecting bacterial membrane potentials
or membrane permeability, or by coagulating the cytoplasm. The
antimicrobial activity of phenolics increases with boiling point,
but so too does their insolubility in water and (in general) their
susceptibility to inactivation by organic matter; high-boilingpoint phenolics tend to be less toxic to tissues. Phenolic disinfectants typically have a high DILUTION COEFFICIENT, and they can
be inactivated by non-ionic surfactants; those which are poorly
soluble in water may be solubilized by alkali or prepared as
suspensions with soaps.
Phenol (carbolic acid, C6 H5 OH) is soluble in water and
(under appropriate conditions) may be bactericidal, fungicidal
and virucidal; its activity against bacterial endospores and acidfast bacteria tends to be very slow. It is toxic to tissues. Phenol
(now produced mainly by chemical synthesis) is used e.g. as a
preservative in animal glues.
In general, alkyl- and halogen-substituted phenolics exhibit
enhanced antimicrobial activity, tend to be less toxic to tissues, and are typically less water-soluble than phenol. In 4alkylphenols, activity increases with alkyl chain length up to
6 carbon atoms. Among halogenated phenols, 4-halophenols are
the most active; in phenolics containing both alkyl and halogen
substituents, activity is maximum when these are in the 2 and 4
positions, respectively. Nitrophenols tend to be more toxic than
other phenolics to tissues. Polyhydric phenols generally have
weak antimicrobial activity. (See also BISPHENOLS.)
Lysol consists of 2-, 3- and 4-cresols (methylphenols) solubilized by soap. Aqueous Lysol (0.5%) kills many non-sporing
pathogens in 15 min, but endospores may survive in 2% Lysol
for several days. Amyl-3-cresol is used e.g. in antiseptic lozenges
and mouthwashes. Sudol consists of xylenols (dimethylphenols) and ethylphenols; it is more active and less corrosive
than Lysol and is active against e.g. staphylococci and tubercle
bacilli. Aqueous Sudol (2%) can inactivate Clostridium perfringens endospores in about 4 hours, but inactivation of Bacillus
subtilis endospores has been found to require 6 hours in a 66%
solution. Hexylresorcinol (4-n-hexyl-1,3-dihydroxybenzene) has
been used as a skin wound cleanser, a urinary antiseptic,
and a constituent of throat lozenges. Menthol (3-methyl-6isopropylphenol) and carvacrol (2-methyl-5-isopropylphenol)
pheromone
are both used in antiseptic lozenges and mouthwashes. Thymol (5-methyl-2-isopropylphenol) is used as a disinfectant, as
an antiseptic (e.g. in mouthwashes), and as a preservative (e.g.
in urine samples pending biochemical tests). 2-Phenylphenol
(2-hydroxydiphenyl) is primarily an antifungal agent but also
has antibacterial activity; it has been used e.g. as a fungicide
in the paper industry, as a preservative in waxed papers, and
as a constituent of PINE DISINFECTANTS. Sodium-o-phenylphenate
is used e.g. for the initial antifungal disinfection of stored
fruits. 2-Benzyl-4-chlorophenol is active against Gram-positive
and Gram-negative bacteria, protozoa and fungi; it is used e.g.
in antiseptic soaps. Chlorocresol (4-chloro-3-methylphenol) is
used e.g. as a preservative for pharmaceutical products and e.g.
for glues and paints. It is also used as a biocide in a lowtemperature (98100 C) STERILIZATION process. Chloroxylenols
(e.g. 4-chloro-3,5-dimethylphenol) are used e.g. as topical antiseptics; they are active ingredients in Dettol. Pentachlorophenol
is used e.g. as a fungicide in wood pulp and as a preservative
for leather, paper and textiles. Picric acid (2,4,6-trinitrophenol),
which has antibacterial and antifungal properties, is also used as
a chemical FIXATIVE. 4-Nitrophenol is used as a preservative in
the leather industry. (See also DINITROPHENOLS.)
(See also BLACK FLUIDS; CREOSOTE; SALICYLIC ACID; WHITE
FLUIDS.)
phenon Any group established on the basis of PHENETIC CLASSIFICATION; in some cases a phenon may be considered to be more
or less equivalent to a TAXON.
phenosafranine A green redox dye see REDOX POTENTIAL.
phenotype The observable characteristics of an organism, either
in total or with respect to one or more particular named characteristics. The phenotype of an organism is the manifestation of
gene expression in that organism. (cf. GENOTYPE.)
phenotypic adaptation See ADAPTATION.
phenotypic lag A delay in the phenotypic expression of a new
allele acquired e.g. by mutation or by gene transfer (e.g.
transduction) due e.g. to SEGREGATION LAG.
phenotypic mixing In a cell simultaneously infected by genetically different viruses: the formation of progeny virions which
either incorporate the genome of one virus within the capsid
of another (transcapsidation or genomic masking) or contain
structural components derived from different parent viruses.
(See also PSEUDOTYPE.)
phenotypic suppression The suppression of a mutant phenotype by non-genetic (environmental) factors. For example, during mRNA synthesis, 5-fluorouracil (5-FU) can be incorporated
instead of uracil and can be misread as cytosine during subsequent translation; thus, e.g., the nonsense codon UAG may
occasionally be misread as CAG (specifying glutamine), thus
simulating a nonsense SUPPRESSOR MUTATION. The accuracy of
translation may also be affected by alteration of ribosomes e.g.
in the presence of STREPTOMYCIN; the resulting mis-reading of
certain codons may lead to the suppression of certain mutations.
phenoxetol See ALCOHOLS.
phenoxyethanol See ALCOHOLS.
b-phenoxyethyldimethyldodecylammonium bromide
Domiphen bromide (see QUATERNARY AMMONIUM COMPOUNDS).
phenoxyethylpenicillin (phenethicillin) A semisynthetic penicillin; R D C6 H5 .O.CH(CH3 ).CO (see b-LACTAM ANTIBIOTICS).
Its activity is similar to that of benzylpenicillin, but it can be
administered orally.
phenoxymethylpenicillin (penicillin V) One of the first natural PENICILLINS to be produced (from P. chrysogenum); in
phenoxymethylpenicillin R D C6 H5 .OCH2 .CO (see b-LACTAM
ANTIBIOTICS).
f
In dioecious species of Achlya, the vegetative female thallus
forms a steroid pheromone (antheridiol, hormone A) which
stimulates the male thallus to form antheridial hyphae; the male
thallus takes up, and inactivates, the pheromone and forms
another steroid pheromone (hormone B) which stimulates the
female thallus to form oogonia.
In some bipolarly heterothallic zygomycetes (e.g. strains
of Blakeslea trispora and Mucor mucedo), development of
sexual structures in the plus and minus mating types (see
HETEROTHALLISM) is governed by trisporic acid derivatives
(formerly referred to as GAMONE) terpene carboxylic acids
synthesized from b-carotene. The plus strains synthesize and
secrete the pheromone prohormone P C (plus-progamone), a
methyldihydrotrisporate; minus strains synthesize and secrete a
trisporol pheromone called prohormone P (formerly minusprogamone). It appears that when each pheromone is taken up
by strains of the opposite mating type it is converted to trisporic
acid in situ. The trisporic acid promotes sexual development and
increases prohormone synthesis.
Pheromones produced by Saccharomyces cerevisiae include
the a-factor and the a-factor (see MATING TYPE). The a-factor is
a tridecapeptide (13 amino acid residues) synthesized as a highMWt precursor (which, interestingly, resembles the hormone
precursors in higher eukaryotes); the precursor is sequentially
cleaved by three proteinases: yscF, yscIV (formerly dipeptidylaminopeptidase A, or X-prolyldipeptidylaminopeptidase), and
(apparently) ysca. The a-factor, an undecapeptide (11 residues),
is apparently also synthesized in precursor form. [MS (1986) 3
107114.]
Algal pheromones. Pheromones are produced by various
algae. In some cases a given pheromone can act on algae
of different genera; for example, among brown algae, the
pheromone ectocarpene (a cyclic hydrocarbon) can act on
Ectocarpus and Sphacelaria, while multifidene is effective in
Chorda and Cutleria. The pheromone desmarestene (structurally
similar to ectocarpene) acts as an attractant to male gametes in
the brown alga Cladostephus [Naturwissenschaften (1986) 73
99100].
f Unwinding angle: see INTERCALATING AGENT.
f6 phage group Syn. CYSTOVIRIDAE.
phialide (phialid) See CONIDIUM.
phialidic development See CONIDIUM.
Phialoascus See ENDOMYCETALES.
Phialophora
A genus of fungi (class HYPHOMYCETES) which
include plant-pathogenic species e.g. P. cinerescens (causal
agent of carnation wilt). (See also CHROMOBLASTOMYCOSIS.)
[Species parasitic on bdelloid rotifers: Mycol. (1984) 76
11071110.] The mycelium is septate, and the conidia (produced from phialides) are non-septate, colourless or pigmented.
(For P. dermatitidis see WANGIELLA.)
phialopore See VOLVOX.
Phialospora See DOTHIDEALES.
Philadelphia chromosome An abnormal human chromosome 22
associated with chronic myelogenous leukaemia: see ABL.
Philaster See SCUTICOCILIATIDA.
Philomiragia bacterium A non-motile bacterium pathogenic in
muskrats. It was formerly called Yersinia philomiragia, but has
been excluded from Yersinia on the basis of DNA homology
studies [Book ref. 22, p. 506].
pHisoHex See BISPHENOLS.
fX phage group Syn. MICROVIRIDAE.
Phlebia See APHYLLOPHORALES (Corticiaceae).
Phlebotomus A genus of blood-sucking sandflies which includes
the vectors of certain diseases.
phosphorescence
is normally present in raw (i.e., untreated) milk, is inactivated
by PASTEURIZATION so that the test determines the efficiency
of the pasteurization process. Milk containing alkaline-buffered
disodium p-nitrophenyl phosphate is incubated at 37 C for
2 hours and then examined (e.g. by colorimetry) for the presence
or intensity of yellow coloration due to p-nitrophenol. A falsepositive result can be obtained if, subsequent to pasteurization,
the milk has been contaminated with phosphatase-producing
organisms.
Enzymic activity may reappear (reactivation) in e.g. cream
which has been treated by HTST pasteurization; reactivation can
be promoted by the addition of MgCl2 .
phosphate box See PHO REGULON.
phosphate-controlled genes See PHO REGULON.
phosphate potential See CHEMIOSMOSIS.
phosphate regulon See PHO REGULON.
phosphatidases Syn. PHOSPHOLIPASES.
phosphatidic acid See LECITHIN.
phosphatidylcholine See LECITHIN.
phosphatidylethanolamine A product of esterification of
ethanolamine (NH2 (CH2 )2 OH) with phosphatidic acid (see
LECITHIN); it occurs e.g. in the CYTOPLASMIC MEMBRANE in many
bacteria.
phosphoadenosine phosphosulphate See PAPS.
phosphoenolpyruvate carboxykinase See Appendix II(b).
phosphoenolpyruvate carboxylase See Appendix II(b).
phosphoenolpyruvate carboxytransphosphorylase See Appendix II(b).
phosphoenolpyruvate-dependent phosphotransferase system
See PTS.
phosphoenolpyruvate synthase See Appendix II(b).
phosphofructokinase See EMBDENMEYERHOFPARNAS PATHWAY.
6-phosphogluconate pathway May refer to either HETEROLACTIC
FERMENTATION or the HEXOSE MONOPHOSPHATE PATHWAY.
phosphoketolase See HETEROLACTIC FERMENTATION.
phospholipases (phosphatidases) Enzymes that hydrolyse phospholipids, releasing fatty acids or other groups (cf. LIPASES).
Phospholipases A1 and A2 release fatty acids from, respectively,
positions 1 and 2 of a phospholipid; phospholipases C and
D release the base in phosphorylated and unphosphorylated
form, respectively from e.g. phosphatidylcholines (lecithins),
sphingomyelins etc. Phospholipases may act specifically (or
preferentially) on particular phospholipids see e.g. LECITHINASE and SPHINGOMYELINASE.
phosphonoacetic acid (PAA) An ANTIVIRAL AGENT (used as disodium phosphonoacetate, D Fosfonet sodium) which is similar
to, but more toxic than, PHOSPHONOFORMIC ACID.
phosphonoformic acid (PFA) An ANTIVIRAL AGENT (used as
trisodium phosphonoformate, NaO.CO.PO.(ONa)2 , D Foscarnet
sodium) which acts by selectively inhibiting the DNA polymerases of a number of viruses (and the reverse transcriptase of
retroviruses) apparently by acting as an analogue of pyrophosphate. It is effective e.g. in the topical treatment of herpesvirus
infections.
phosphonomycin Syn. FOSFOMYCIN.
phosphorelay See ENDOSPORE (sense 1).
phosphorescence (1) The emission of light which occurs when
certain substances absorb radiation; emission occurs as electrons
excited to the triplet state (T1 ) are returning to the (unexcited)
ground state (S0 ). The light emitted is of wavelength longer
than that of the exciting radiation; emission typically lasts for
106 sec to 1 sec or longer. (cf. FLUORESCENCE.) (2) The term
is sometimes applied, incorrectly, to BIOLUMINESCENCE.
phosphoribulokinase
under aerobic conditions; this effect appears to be due largely
to the formation of SINGLET OXYGEN [JAB (1985) 58 391400].
ETHIDIUM BROMIDE can cause a light-induced nicking of DNA.
photoheterotroph A phototrophic HETEROTROPH.
photoinduction and photoinhibition (in fungi) In many fungi,
light is needed for, or encourages, the development of fruiting
bodies or spores, or the formation of particular compounds (photoinduction); in other fungi light inhibits growth and/or sporulation (photoinhibition). Commonly, light in the blue-violet region
of the spectrum is effective in photoinduction/photoinhibition.
In some cases light may be needed only for the completion
of a particular phase of development, e.g., the initiation of
fruiting in Pyronema omphalodes, or the development of the
pileus in Lentinus lepideus (cf. STAGS HORN FUNGUS). Conidium
formation is photoinducible in e.g. Trichoderma viride, and
in Choanephora cucurbitarum it is stimulated by darkness
preceded by a period of exposure to light. In some species of
Coprinus fruiting bodies develop more rapidly in the light, i.e.,
light encourages fruiting but is not essential for it. In Phycomyces
blakesleeanus carotenoid synthesis is stimulated by light, while
some species of Fusarium and Verticillium which normally form
negligible amounts of carotenoids form significant amounts of
these compounds in the presence of light.
Photoinhibition of growth and/or sporulation occurs e.g. in
at least some species of Alternaria and Penicillium. In e.g.
Alternaria cichorii, A. tomato and Botrytis cinerea, conidium
formation is controlled by a photoreceptor system referred to as
mycochrome. On exposure to blue light mycochrome adopts the
MNUV form, in the presence of which conidia are not formed
and conidiophores may revert to vegetative hyphae; on exposure
to near-ultraviolet mycochrome adopts the MB form, in the
presence of which conidia can be formed. In A. cichorii the
blue-light inhibition of conidium formation can be reversed by
a period of darkness [CJB (1986) 64 10161017].
photoinhibition See PHOTOINDUCTION AND PHOTOINHIBITION.
photokinesis A KINESIS (sense 1 or 2) in which the stimulus is
light intensity.
photolithotroph See LITHOTROPH.
photolyase In some bacteria (including Escherichia coli ): an
enzyme which can repair thymine dimers in DNA damaged by
ULTRAVIOLET RADIATION; the energy needed for repair is derived
from (visible) light. In vitro studies on the repair of thymine
dimers may be facilitated by using the reagent potassium
permanganate (KMnO4 ) [NAR (1998) 26 39403943].
photomicrograph A photograph obtained by PHOTOMICROGRAPHY.
photomicrography Photography of microscopic objects through
a microscope; it may involve the attachment of a camera to
a microscope, or the use of a photomicroscope: a microscope
which incorporates a camera. (cf. MICROPHOTOGRAPHY.)
photomicroscope See PHOTOMICROGRAPHY.
photomorphogenesis The formation of new cells or tissues under
the stimulus of light.
photoorganotroph See ORGANOTROPH.
photophobic response A light-induced PHOBIC RESPONSE.
photophosphorylation See PHOTOSYNTHESIS and PURPLE MEMBRANE.
photoreactivation (photorestoration) A mechanism of DNA
REPAIR in which pyrimidine dimers (formed as a result of exposure to ULTRAVIOLET RADIATION) are cleaved by exposure of the
cells to light of wavelength ca. 300600 nm; in Escherichia
coli the reaction is mediated by the product of the phr gene
(DNA photolyase) which, when bound to a pyrimidine dimer,
photosynthesis
photorestoration Syn. PHOTOREACTIVATION.
photosynthate Any carbohydrate product of photosynthesis.
photosynthesis In certain (photosynthetic) organisms: the process in which radiant energy is absorbed by specialized
CHLOROPHYLL-containing pigment system(s) and is converted
to forms of energy (including chemical energy) which can
be used for metabolic and other purposes (cf. PURPLE MEMBRANE); radiation of wavelengths in the visible spectrum is
used by plants, ALGAE and photosynthetic bacteria (including
CYANOBACTERIA and members of the RHODOSPIRILLALES), while
some photosynthetic bacteria can also use infrared radiation.
Light reaction refers, collectively, to those photochemical events
involved in the conversion of radiant energy; dark reaction
(D light-independent reaction) generally refers, collectively, to
those reactions in which photosynthetically derived chemical
energy is used for the synthesis of carbohydrate(s).
In all cases, the conversion of radiant energy occurs
in a specialized ENERGY-TRANSDUCING MEMBRANE containing
CHLOROPHYLLS or bacteriochlorophylls, accessory pigments, and
components of ELECTRON TRANSPORT CHAIN(S). Within such a
photosynthetic membrane there are well defined chlorophyllcontaining REACTION CENTRES towards which radiant energy is
channelled via LIGHT-HARVESTING COMPLEXES. On excitation of a
reaction centre with radiant energy, the mid-point REDOX POTENTIAL of the reaction centre chlorophyll changes from a high
positive value to a high negative value, and electrons are consequently ejected (charge separation) from the chlorophyll (the
primary electron donor). The ejected electrons, by virtue of the
high negative redox potential of their source, are associated with
a certain amount of energy; these electrons can therefore pass
down an electron transport chain in the direction of less negative
(or more positive) potentials and, in doing so, can provide the
energy for (a) the transmembrane pumping of protons (thereby
contributing to a proton motive force see CHEMIOSMOSIS) or (b)
the reduction of pyridine nucleotides. The precise nature of photosynthetic energy conversion differs among the different groups
of photosynthetic organisms.
(a) Photosynthesis in bacteria of the Rhodospirillales (anoxygenic photosynthesis) occurs only under anaerobic conditions,
and only one type of reaction centre appears to occur in a given
species.
In the purple photosynthetic bacteria (RHODOSPIRILLINEAE),
electrons which have been ejected from the bacteriochlorophyll
follow a cyclic path: e.g. from the bacteriochlorophyll to BACTERIOPHAEOPHYTIN and thence probably via QUINONES, b-and
c-type cytochrome(s) back to the reaction centre; this cyclic
electron flow causes the transmembrane pumping of protons,
i.e., it generates pmf. The pmf can be used, by means of
membrane-bound PROTON ATPASES, for the synthesis of ATP (photophosphorylation). At least some of these organisms can obtain
reducing power by REVERSE ELECTRON TRANSPORT; in this process, photosynthetically generated pmf is used to reduce NADC
at a membrane-bound NADH dehydrogenase electrons being
obtained from an external electron donor (such as hydrogen or
sulphide). NADPH is obtained via a TRANSHYDROGENASE.
In the green photosynthetic bacteria (CHLOROBIINEAE), the
light-energized reaction centre reaches a much lower (more
negative) potential (ca. 550 mV) than is the case in the purple
bacteria, and consequently the ejected electrons are able to
effect the reduction of NADC (the Em,7 of the NADC /NADH
redox couple being 320 mV); the reduction of NADC involves
a non-cyclic electron transport path which is believed to include
ironsulphur proteins. Electrons which are removed from the
absorbs light energy and cleaves the bonds between the bases
(monomerization). [Action mechanism of E. coli DNA photolyase: JBC (1987) 262 478485, 486491, 492498.] The
phr gene product may also play a role in UvrABC-dependent
repair of UV damage in the dark [JB (1985) 161 602608].
Photoreactivation does not occur e.g. in Bacillus subtilis.
photoreceptor An organelle or region specialized for receiving
light stimuli: see e.g. EYESPOT (sense 1), STENTORIN and STENTOR.
photoreduction In photosynthetic organisms (see PHOTOSYNTHESIS): any light-dependent reduction e.g., the reduction of
NADC , or of CO2 via the Calvin cycle; electron donors used in
photoreductions include e.g. water and H2 S.
In certain algae (e.g. Chlorella, Chlamydomonas, Scenedesmus)
hydrogen can act as electron donor for the reduction of CO2 ;
HYDROGENASE is involved, and the process can occur only after the
algae have been incubated anaerobically with hydrogen, followed
by illumination with low levels of light.
photorespiration (C2 carbon oxidation cycle) In photosynthetic
organisms which fix CO2 via the CALVIN CYCLE: a lightdependent process in which oxygen is consumed and CO2
is evolved, but which is distinct from true (energy-yielding)
RESPIRATION; photorespiration occurs under conditions of relatively high O2 and low CO2 concentrations and high light
intensities, and results from the ability of RIBULOSE 1,5BISPHOSPHATE CARBOXYLASEOXYGENASE (RuBisCO) to act as
an oxygenase under these conditions. RuBisCO catalyses the
oxygenation and cleavage of ribulose 1,5-bisphosphate (RuBP)
to 3-phosphoglycerate and 2-phosphoglycolate. (The dependence
of photorespiration on light is thus explained by the need for
photosynthesis to drive the CALVIN CYCLE and hence supply
RuBP.) The 2-phosphoglycolate is dephosphorylated to glycolate which may be excreted e.g. by certain microalgae and
cyanobacteria (often resulting in relatively high levels of glycolate in aquatic environments) and/or may be metabolized
further: e.g. glycolate ! glyoxylate ! glycine ! serine !
hydroxypyruvate ! glycerate ! 3-phosphoglycerate (the glycolate pathway). The step glycolate ! glyoxylate is also an
O2 -consuming step (catalysed by glycolate oxidase); H2 O2 generated during the reaction is rapidly degraded by catalase.
(The glycolate ! glyoxylate conversion occurs in PEROXISOMES
in photosynthetic eukaryotes.) The 3-phosphoglycerate generated by the glycolate pathway and by the original cleavage
of RuBP by RuBisCO may then enter the Calvin cycle. An
alternative pathway for glycolate metabolism in some organisms involves the oxidation of glycolate to glyoxylate which is
then converted to glycerate via tartronic semialdehyde (TSA).
In either pathway, CO2 is lost: in the glycolate pathway during the glycine ! serine reaction (during which two glycine
molecules are converted to one of serine with loss of both CO2
and NH3 ), and in the TSA pathway during the formation of
TSA from glyoxylate (2CHO.COOH ! CHO.CHOH.COOH C
CO2 ). Photorespiration thus results in a net loss of photosynthetic productivity. Its physiological significance is still not
understood. In green algae, photorespiration is suppressed by
CO2 -concentrating mechanisms which become operative at low
CO2 levels. [Review of photorespiration: ARPphys (1984) 35
415442.] (cf. WARBURG EFFECT.)
A process very similar to photorespiration (although independent of light) occurs in some chemolithoautotrophic bacteria
(e.g. Alcaligenes eutrophus, Thiobacillus neapolitanus) which
fix CO2 via the Calvin cycle; by analogy with photorespiration,
this process has been called chemorespiration. [Book ref. 115,
pp. 129173.]
581
photosynthesis
photosystem II
photosystem I
(PS-II)
(PS-I)
P*700
1.0
iron-sulphur
proteins
P*680
E m(volts)
0.5
ferredoxin
phaeophytin
quinones
NADP
cytochrome
b6 / f
complex
light
plastocyanin
P700
0.5
H2O
2e
1.0
1
2
light
P680
O2 + 2H+
PHOTOSYNTHESIS. Simplified Z scheme for non-cyclic, oxygenic photosynthetic electron transport (scale approximate). Each photosystem
(PS-I and PS-II) consists of a reaction centre together with its associated accessory pigments. P680 and P700 represent the chlorophylls in the
reaction centres of PS-II and PS-I, respectively; P680 and P700 represent the excited state in P680 and P700 , respectively. The cytochrome b6 /f
complex includes cyts b6 and f, quinone, and a Rieske ironsulphur protein.
phycobilisomes
Phragmobasidiomycetidae A subclass of fungi (class HYMENOMYCETES) characterized by the formation of phragmobasidia (see
BASIDIUM). Orders [Book ref. 64, p. 189]: AURICULARIALES, SEPTOBASIDIALES, TREMELLALES.
phragmobasidium See BASIDIUM.
phragmoplast In e.g. some green algae (e.g. Chara): a plate
which develops in the cleavage plane between two newly
forming cells during the telophase stage of MITOSIS; it consists of
microtubules of the persistent mid-region of the mitotic spindle
together with vesicles (derived from dictyosomes) which collect
between the microtubules. (cf. PHYCOPLAST.)
phragmosporae See SACCARDOAN SYSTEM.
phthalimide antifungal agents A group of agricultural nonsystemic ANTIFUNGAL AGENTS which includes CAPTAFOL, CAPTAN,
FOLPET etc.
phthalylsulphathiazole See SULPHONAMIDES.
phthiocerols Complex waxes found in mycobacteria [JGM
(1983) 129 859863].
phthisis Syn. TUBERCULOSIS.
phycobilin See PHYCOBILIPROTEINS.
phycobiliproteins (biliproteins) Water-soluble pigments which
occur in CYANOBACTERIA, in algae of the RHODOPHYTA, and in
CRYPTOPHYTES. In cryptophytes the pigments occur between the
thylakoids and are antigenically unrelated to the cyanobacterial and rhodophytan pigments (which occur bound to thylakoids see PHYCOBILISOMES). A phycobiliprotein consists
of a protein monomer comprising two distinct polypeptide chains (a and b), each of which is linked covalently
(via a thioether bond) to an open-chain tetrapyrrole chromophore (phycobilin or bilin). The monomers tend to form
trimers or hexamers which are the structural units of phycobilisomes. Phycobiliproteins function as light-harvesting pigments for photosystem II (see PHOTOSYNTHESIS); there are three
main classes: allophycocyanins (lmax 650671 nm), phycocyanins (lmax 617620 nm), and phycoerythrins (including
phycoerythrocyanin: lmax 545568 nm). Allophycocyanins and
phycocyanins apparently occur in all cyanobacteria and red
algae; phycoerythrins occur in most red algae and in many
cyanobacteria, phycoerythrocyanin occurs in some cyanobacteria
(e.g. Anabaena variabilis, Mastigocladus laminosus ). Cryptophytes contain either phycocyanin or phycoerythrin, according to
species. In cyanobacteria, the content of phycobiliproteins can
be affected by many environmental factors, including temperature, CO2 concentration, nitrogen starvation, wavelength and
intensity of light [Book ref. 76, pp. 182188]; in addition to its
function as a photopigment, phycocyanin serves as a nitrogen
reserve in cyanobacteria, being degraded by a specific protease induced during nitrogen starvation both in vegetative cells
and in differentiating HETEROCYSTS. [Structure and function of
cyanobacterial phycobiliproteins: Book ref. 75, pp. 2342; the
phycocyanin operon and light regulation of its expression in
Anabaena: EMBO (1987) 6 871884.]
phycobilisomes Structures, each ca. 2070 nm across, which are
attached in regular arrays to the surface of thylakoid membranes in CYANOBACTERIA (cf. GLOEOBACTER) and red algae
(RHODOPHYTA). Phycobilisomes are composed mainly of PHYCOBILIPROTEINS together with linker polypeptides; they vary
in composition and morphology (being typically hemidiscoid
or hemispherical) according e.g. to species. The (mainly nonpigmented) linker polypeptides seem to have many functions e.g. to stabilize the specific structure of phycobilisomes,
to modify the phycobiliproteins so as to promote unidirectional
phycobiont
energy flow within the phycobilisomes and to the reaction centres, and to link phycobilisomes to the photosynthetic membranes.
In general, each phycobilisome comprises two major structural
domains: (i) a core (consisting of two or three cylindrical elements), and (ii) five or six rods (composed of stacked discs)
that radiate from the core to form the hemidiscoid or hemispherical structure. The core is composed of allophycocyanin
(APC) and is anchored to the thylakoid membrane by a linker
polypeptide. Where the rods are adjacent to the core, they consists of discs of phycocyanin (PC), but discs of phycoerythrin
(PE) and/or phycoerythrocyanin (PEC), when present, occur at
the periphery.
Absorbed light energy is transferred from the periphery to the
core, and thence to chlorophyll a thus: PE/PEC ! PC !
APC ! Chl a; this transfer is almost 100% efficient.
[Structure of a simple phycobilisome (in Synechococcus):
Ann. Mic. (1983) 134 B 159180. Phycobilisome structure: JB
(1993) 175 575576.]
phycobiont An algal symbiont. In lichenology, phycobiont
commonly refers to the main algal or cyanobacterial partner
in a lichen, although in the latter case the term cyanobiont is
more appropriate. The term photobiont is a useful non-specific
term for the principal photosynthetic partner in a LICHEN. (See
also PHYCOZOAN.)
phycocyanins See PHYCOBILIPROTEINS.
phycoerythrins See PHYCOBILIPROTEINS.
phycoerythrocyanin See PHYCOBILIPROTEINS.
phycology The study of ALGAE.
Phycomyces See MUCORALES.
phycomycetes See LOWER FUNGI.
phycomycosis See ZYGOMYCOSIS and EQUINE PHYCOMYCOSIS.
Phycopeltis A genus of algae closely related to TRENTEPOHLIA.
The thallus is typically a circular monostromatic disc (ca.
13 mm diam.) of compacted, branched filaments. Species occur
mainly as epiphytes, growing on not beneath the leaf cuticle
(cf. CEPHALEUROS), and also as photobionts in certain (mainly
tropical) lichens.
phycoplast In many green algae: a plate which develops in the
cleavage plane between two newly forming cells in species
in which the mitotic spindle is non-persistent; it contains
microtubules orientated perpendicular to the axis of the former
spindle. (cf. PHRAGMOPLAST.)
phycosymbiodeme See CEPHALODIUM.
phycotoxin Any TOXIN produced by an alga (see e.g. BREVETOXINS, CIGUATERA, GONYAUTOXINS, PRYMNESIUM, SAXITOXIN, ULVA)
or traditionally by a cyanobacterium (blue-green alga: see
e.g. ANABAENA, APHANIZOMENON, LYNGBYA, MICROCYSTIS, NODULARIA).
phycovirus A VIRUS which infects one or more ALGAE. (cf.
CYANOPHAGE.) Several polyhedral dsDNA viruses have been
observed in green algae: e.g. a tailed polyhedral virus, resembling (at least superficially) a tailed bacteriophage, has been
found in Uronema gigas [Virol. (1980) 100 156165, 166174],
and various polyhedral dsDNA viruses have been observed in
Chlorella-like algae, including the zoochlorellae of Paramecium
bursaria and Hydra viridis [PNAS (1982) 79 38673871].
phycozoan A term proposed to refer to a compound organism
in which cells (or chloroplasts) of an alga (the phycobiont)
live within the tissues or cells of an animal (the zoobiont: an
invertebrate) [Book ref. 129, pp. 517].
(See e.g. ZOOCHLORELLAE and ZOOXANTHELLAE; cf. LICHEN.)
phyletic classification Syn. PHYLOGENETIC CLASSIFICATION.
Phytophthora
certain (pathogenic and non-pathogenic) microorganisms or to
heavy metals (e.g. copper, mercury), detergents or certain other
chemicals, ultraviolet radiation or physical (e.g. freezethaw)
damage. Phytoalexins are formed by many angiosperms (particularly by members of the Leguminosae and Solanaceae) and
by some gymnosperms; they have not been detected in lower
plants.
Under pre-stimulus conditions, phytoalexins may be either
absent from plant tissues or present in extremely low concentrations.
The production of phytoalexins appears to be a local effect
in the plant their translocation has yet to be conclusively
demonstrated; if phytoalexins are involved in a plants natural
resistance to disease, their localized accumulation may be an
important factor in such resistance. In some cases the ability
to produce phytoalexin(s) appears to enable a plant to resist
the development of disease following infection by a pathogen;
thus, e.g. resistance of the French bean to Colletotrichum
lindemuthianum seems to correlate with the accumulation of
a phytoalexin, phaseollin. In other cases the accumulation of
phytoalexins appears not to be the sole factor which determines
the plants resistance to disease. Pathogens which are able
successfully to invade a plant may (i) fail to induce the
production of phytoalexins; (ii) be relatively insensitive to the
phytoalexin(s) produced; or (iii) be able to convert a phytoalexin
to an inactive form (see e.g. KIEVITONE and PISATIN). (See also
HYPERSENSITIVITY sense 2.)
Elicitors of phytoalexins, i.e. specific chemical entities which
promote the synthesis of phytoalexins, include the polypeptide
monilicolin A (which elicits PHASEOLLIN) and various polysaccharides (such as b-1,3- and b-1,6-glucans and CHITOSAN) present
e.g. in fungal cell walls or culture filtrates. Physical damage
to plant tissues may cause release of the plants own elicitors
(constitutive or endogenous elicitors). [Phytoalexins and their
elicitors: ARPphys. (1984) 35 243275.]
Phytoalexins are structurally/chemically diverse compounds;
they include e.g. CAMALEXIN; CAPSIDIOL; DEOXYHEMIGOSSYPOL;
FALCARINDIOL; GLYCEOLLIN; HIRCINOL; IPOMEAMARONE; KIEVITONE; LUBIMIN; MOMILACTONES (see also WL 28325); ORCHINOL; PHASEOLLIN; PISATIN; PTEROSTILBENE; RISHITIN; VIGNAFURAN;
VINIFERINS; and WYERONE.
(cf. AVENACIN; CAFFEIC ACID; CHLOROGENIC ACID; PATHOGENESISRELATED PROTEINS.)
[Phytoalexins (structure, role etc.): ARPpath. (1999) 37
285306.]
phytobiont A plant symbiont e.g. the plant partner in a MYCORRHIZA.
phytoflagellates See PHYTOMASTIGOPHOREA.
phytoflavin See FLAVODOXINS.
phytoglycogen A type of GLYCOGEN-like polysaccharide found
e.g. in certain algae. (cf. CYANOPHYCEAN STARCH.)
phytohaemagglutinin (PHA) (1) A mitogenic LECTIN from the
red kidney bean, Phaseolus vulgaris; it can agglutinate erythrocytes, and it binds to both B and T cells but is mitogenic mainly
in T cells. PHA activity requires Ca2C and Mg2C and is inhibited
e.g. by N-acetyl-D-galactosamine. (2) Any plant lectin which can
agglutinate erythrocytes.
phytohormones (plant hormones) Compounds which are produced by plants and which regulate the plants own metabolism,
cell division, seed germination etc; they include ABSCISIC ACID,
AUXINS, CYTOKININS, ETHYLENE and GIBBERELLINS.
phytokinins See CYTOKININS.
phytoplankton
olives and cucumbers cf. SAUERKRAUT). [Lactic acid bacteria
in vegetable fermentations: Food Mic. (1984) 1 303313.]
Fermentative yeasts may also be present; these may ferment any
sugars remaining after the lactic acid bacteria have been inhibited
by acidity. The combination of salt, anaerobiosis and low pH
serves to discourage the growth of undesirable organisms.
Microbial spoilage of pickled vegetables may be due e.g. to
oxidative pectinolytic moulds and yeasts which cause softening
of the vegetable tissue; these organisms form a surface film
unless precautions are taken to exclude air. Oxidative yeasts may
also metabolize lactic acid and hence reduce acidity, allowing
the subsequent growth of other spoilage organisms. Spoilage
bacteria (e.g. coliforms, clostridia) tend to grow when the pH
is too high and/or the salt concentration too low; they can
cause softening, off-flavours and odours, and/or the formation
of gas pockets within the vegetable (called bloater damage in
cucumbers, fisheye spoilage in olives).
picodnaviruses Rejected name for the PARVOVIRIDAE.
a-picolinic acid Pyridine 2-carboxylic acid, a toxin produced by
Pyricularia oryzae. (See also BLAST DISEASE and PIRICULARIN.)
Picornaviridae A family of small, ssRNA-containing VIRUSes in
which the icosahedral virion (ca. 2230 nm diam.) is naked
and ether-resistant. Most picornaviruses have a narrow host
range, and some are important pathogens of man and animals;
transmission generally occurs mechanically. The family includes
four genera: APHTHOVIRUS, CARDIOVIRUS, ENTEROVIRUS and RHINOVIRUS; within the genera, species are distinguished by their
susceptibility to specific neutralizing antibodies. Some picornaviruses are currently not classified into genera; these include
equine rhinovirus types 1 and 2, and insect picornaviruses such
as cricket paralysis virus, Drosophila C virus and Gonometa
virus. Possible picornaviruses include unclassified small RNA
viruses of invertebrates: e.g., bee acute paralysis virus, bee slow
paralysis virus, bee virus X, black queen cell virus, Drosophila
P and A viruses, FLACHERIE virus and SACBROOD virus. [Review
of small RNA viruses of insects: JGV (1985) 66 647659.]
Virion structure. The capsid comprises 60 subunits, a subunit
consisting of one molecule each of the 4 major capsid polypeptides (VP1VP4); portions of VP1, VP2 and VP3 are exposed
at the virion surface, while VP4 is probably internal and may
be associated with the RNA. [Virion structure in polioviruses:
Science (1985) 229 13581365, and in rhinoviruses: Nature
(1985) 317 145153.] The RNA genome is a single molecule
of linear positive-sense ssRNA (MWt ca. 2.5 106 ) which is
polyadenylated at its 30 end and covalently linked at its 50
end to a virus-encoded protein, VPg. In cardioviruses and aphthoviruses (but not in enteroviruses or rhinoviruses) the RNA
contains a poly(C) tract near the 50 end, the length of which
varies with strain. [Poly(C) secondary structure in aphthoviruses:
JGV (1985) 66 19191929.]
Replication cycle. Virus replication occurs in the host cell
cytoplasm. Infection begins when a virion attaches to receptors
in the host cell plasma membrane; in e.g. poliovirus type 1 and
mouse Elberfeld virus, entry into the host cell apparently occurs
by endocytosis, and uncoating apparently occurs in endosomes
and/or lysosomes [JGV (1985) 66 483492]. In polioviruses,
translation of the viral RNA is initiated at one site near the 50
end of the RNA, resulting in the formation of a polyprotein;
the polyprotein is initially cleaved, during translation, into
three precursor proteins (P1, P2 and P3), each of which
undergoes further cleavage. P1 gives rise to 1A, 1B, 1C and
1D (capsid polypeptides); P2 gives rise to 2A, 2B (a host-range
determinant), and 2C (involved in RNA synthesis); P3 undergoes
pili
intramolecular self-cleavage to form 3A, 3B (VPg), 3C (a
protease which carries out most of the proteolytic cleavages),
and 3D (an RNA polymerase which can elongate nascent RNA
chains on an RNA template). [Nomenclature of picornavirus
proteins: JV (1984) 50 957959.] In contrast to polioviruses,
aphthoviruses have two distinct translation initiation sites [JGV
(1985) 66 26152626].
Replication of the RNA genome is associated with the smooth
endoplasmic reticulum; ()-strand synthesis may involve a
primer formed by hairpin folding of the (C)-strand template,
resulting in a product up to twice the length of the genome (at
least in vitro) [JV (1986) 58 790796].
Virus assembly is preceded by cleavage of P1 to form an
immature 5S protomer containing VP0, VP1 and VP3. The
immature protomers become associated with an RNA genome
to form a provirion. During maturation most or all of the
VP0 molecules are cleaved to form VP2 and VP4. The mature
virions are eventually released by host cells lysis. (Some
picornaviruses e.g. hepatitis A virus can cause non-lytic
infections.)
Most picornaviruses can be propagated in cell cultures.
Infected cells undergo drastic changes in their macromolecular
metabolism: the rate of RNA synthesis declines shortly after
infection, and cellular protein synthesis is inhibited soon after.
[Review of inhibition of protein synthesis: Book ref. 150,
pp. 177221.] Characteristic CPEs generally develop in the
infected cells: e.g., accumulation of chromatin on the inside
of the nuclear envelope; appearance of membranous vesicles
in the cytoplasm; formation of crystalline arrays of virions in
the cytoplasm; alterations in membrane permeability leading to
shrivelling of the cell; etc.
picornaviruses Viruses of the PICORNAVIRIDAE.
picric acid (2,4,6-trinitrophenol) An antimicrobial agent (see
PHENOLS), a fixative (see e.g. BOUINS FLUID), and a DYE.
piedra See BLACK PIEDRA and WHITE PIEDRA.
Piedraia
A genus of fungi of the DOTHIDEALES (anamorph:
Trichosporon). (See BLACK PIEDRA.)
piericidin An antibiotic, produced by Streptoverticillium mobaraense, which acts as a RESPIRATORY INHIBITOR in mitochondrial
and bacterial ELECTRON TRANSPORT CHAINS (although intact cells
may be impermeable and hence insensitive to piericidin); the
(non-covalent) binding site(s) and mechanism of action of
piericidin are apparently similar to those of ROTENONE.
pif A locus in the F PLASMID associated with the inability of
certain phages (e.g. T7) to replicate in cells containing the
F plasmid. (pif D phage-inhibitory function.) (See also FEMALESPECIFIC PHAGE.)
pig bel Syn. ENTERITIS NECROTICANS.
pig diseases (a) Bacterial diseases: see e.g. EPERYTHROZOONOSIS, FOOT-ROT, GLASSERS DISEASE, GREASY PIG DISEASE, OEDEMA
DISEASE, PARATYPHOID FEVER (sense 2), SWINE DYSENTERY, SWINE
ERYSIPELAS, TULARAEMIA. (b) Viral diseases: see e.g. AFRICAN
SWINE FEVER, AUJESZKYS DISEASE, FOOT AND MOUTH DISEASE,
INCLUSION BODY RHINITIS, PARVOVIRUS, SWINE FEVER, SWINE
INFLUENZA, SWINE POX, SWINE VESICULAR DISEASE, TALFAN DISEASE, TESCHEN DISEASE, TRANSMISSIBLE GASTROENTERITIS, VESICULAR EXANTHEMA, VESICULAR STOMATITIS, VOMITING AND WASTING
DISEASE.
pigeonpox virus See AVIPOXVIRUS.
pil genes
The designation of genes which encode type IV
FIMBRIAE in various Gram-negative bacteria e.g. Neisseria
gonorrhoeae and Pseudomonas aeruginosa; for example, in
N. gonorrhoeae, pilC encodes the terminal adhesin, pilE encodes
587
Pilimelia
bacteria, but were poorly active against Gram-positive species.
Modern pine fluids (with RW coefficients of ca. 35) typically
contain phenolics (e.g., 2-phenylphenol, 4-chloro-3,5-xylenol)
together with e.g. terpineol (an antimicrobial constituent of pine
oil) and a solubilizing agent, e.g., potassium ricinoleate; these
fluids are active against both Gram-negative and Gram-positive
bacteria. The activity of at least one pine fluid against Pseudomonas aeruginosa is greatly increased at temperatures above
30 C [Book ref. 13, pp. 8590]. The recommended maximum
dilution of a pine fluid is 20 times its RW coefficient.
pink-eye (pinkeye) (1) Syn. CONJUNCTIVITIS. (2) An acute contagious conjunctivitis caused by Haemophilus aegyptius. (3) Syn.
INFECTIOUS KERATITIS (of cattle).
Pinnularia See DIATOMS.
pinocytosis The ingestion, by various types of eukaryotic cell
(e.g. amoebae, macrophages), of minute droplets of fluid; in
pinocytosis (as in PHAGOCYTOSIS) a small region of the CYTOPLASMIC MEMBRANE invaginates and is subsequently pinched off
to form a closed, intracellular membranous sac (pinocytotic
vesicle, pinosome) containing the ingested fluid. In one form
of pinocytosis (fluid-phase pinocytosis) pinocytotic vesicles are
formed continually at non-specific sites in the cytoplasmic membrane samples of extracellular fluid being taken randomly;
such vesicles often fuse with LYSOSOMES.
Receptor-mediated pinocytosis (D absorptive pinocytosis) is
a selective process in which specific types of macromolecule
(or e.g. virus particle) are taken up. The macromolecules bind
to specific receptors located at the outward-facing surface of
the cytoplasmic membrane, groups of such receptors occurring
in discrete regions of the cytoplasmic membrane known as
coated pits; a coated pit bears on its inner (i.e., cytoplasmic)
surface a characteristic array of molecules of the fibrous protein
clathrin (MWt ca. 215000). Clathrin occurs in propeller-shaped
(three-legged) trimeric units (triskelions) which assemble into
pentagons and hexagons, forming a polygonal network which
comprises the cytoplasmic face of the coated pit. (Often, bundles
of ACTIN microfilaments stress fibres occur in the cytoplasm
beneath a coated pit.) Following receptor-mediated binding of
macromolecules to a coated pit, the coated pit region invaginates
and eventually pinches off to form a pinocytotic vesicle the
outer (cytoplasm-facing) surface of the vesicle being covered by
a lattice-like network of clathrin; the vesicle, enclosed within
its clathrin cage, is called a coated vesicle. Before fusing with
e.g. a lysosome, a coated vesicle must have its clathrin removed
in an ATP-dependent process. [Enzymatic recycling of clathrin
from coated vesicles: Cell (1986) 46 59.]
pinosome See PINOCYTOSIS.
pinosylvin 3,5-Dihydroxy-trans-stilbene: an antifungal compound formed by many species of pine (Pinus); it appears to
be at least partly responsible for the relative resistance of pine
heartwood to fungal attack. (See also TIMBER PRESERVATION.)
pinta (mal del pinto; syn. spotted sickness) A chronic infectious
human disease caused by Treponema carateum; it occurs in
Central and South America. Symptoms: spots or patches of
abnormally pigmented or depigmented skin; other tissues are
rarely affected. Chemotherapy: e.g. penicillins.
pInv plasmid See EIEC.
pionnotes In Fusarium spp: a flat spore mass which has a fat-like
or greasy appearance.
pipemidic acid See QUINOLONE ANTIBIOTICS.
Piptocephalis A genus of fungi (order ZOOPAGALES) which are
parasitic on other fungi, often other zygomycetes. The vegetative hyphae develop extracellularly on the host from which
plague
vesicle) appears on each side of the plug; the cytoplasmic
membrane thus remains continuous from one cell to another.
(cf. PLASMODESMA.) A secondary pit connection may develop
between two cells which have become juxtaposed. (See also
CHOREOCOLAX.)
pitch canker A disease of pine trees (Pinus spp) caused by
Fusarium moniliforme var. subglutinans; symptoms include
dieback of terminal and lateral branches, and the formation of
CANKERS characterized by a copious flow of resin.
Pitelka convention A system for numbering the microtubular
triplets in a kinetosome. Looking at a cross-section of a
ciliary kinetosome from the direction of the interior of the
cell, the triplet associated with the ribbon of POST-CILIARY
MICROTUBULES is designated number 5; the numbering sequence
is clockwise as in the GRAIN CONVENTION.
Pithomyces See HYPHOMYCETES; see also SPORIDESMINS.
pitted keratolysis A human skin disease characterized by focal
erosion of the stratum corneum, usually on the soles and heels
of the feet; it appears to be caused by an organism resembling
Dermatophilus congolensis.
Pittsburg pneumonia agent Legionella micdadei.
pityriasis nigra (tinea nigra) A benign superficial human dermatomycosis in which brownish or black macules are formed
(usually on the palms of the hands). Causal agents: Exophiala
werneckii (D Cladosporium werneckii ) or Stenella araguata (D
Cladosporium castellanii ).
pityriasis versicolor (tinea versicolor) A mild, chronic, superficial human dermatomycosis caused by Malassezia furfur (Pityrosporum orbiculare); flat or slightly raised, scaly, brownish
or fawn spots (which gradually enlarge and coalesce) develop
mainly on the chest, back, arms and neck. Lesions may fluoresce
greyish-yellow under Woods lamp.
Pityrosporum Syn. MALASSEZIA.
pivampicillin See PENICILLINS.
Pixuna virus See ALPHAVIRUS.
plague
PLAGUE: areas where endemic plague is known to have persisted near the end of the 20th century. Areas in black are regions in which there
are populations of wild rodents that carry the plague bacillus.
Reproduced from Medical Microbiology 14th edition, Figure 36.1, page 406, David Greenwood, Richard Slack & John Peutherer (eds) (1992)
copyright Churchill Livingstone (Harcourt Publishers Ltd, Edinburgh) (ISBN 0-443-04256-X) by courtesy of the author, Dr J. D. Coghlan, and
with permission from the publisher.
plant viruses
the latter bearing elongated sporangia, singly or in groups,
each sporangium containing a serially-arranged pair of spores;
liberated spores become motile (flagellated). Type species:
P. longispora. [Book ref. 73, pp. 111112.]
Planococcus A genus of Gram-positive, asporogenous, catalasepositive, chemoorganotrophic, aerobic bacteria which occur as
marine saprotrophs. Cells: cocci (each having 13 flagella)
which occur in pairs and tetrads; the cell wall contains no teichoic acids. A yellow-brown pigment is formed. Carbohydrates
are not utilized. Growth occurs e.g. on nutrient agar containing
12% NaCl. GC%: ca. 3951. Species: P. citreus (type species)
and P. halophilus.
planofluorite See FLUORITE OBJECTIVE.
planogamete A motile GAMETE.
Planomonospora A genus of bacteria (order ACTINOMYCETALES,
wall type III; group: maduromycetes) which occur in soil. The
organisms form branching substrate and aerial mycelium, the
latter bearing rows of parallel, elongated sporangia, each sporangium being attached at one end to the hypha; each sporangium contains one spore which becomes motile (flagellated)
after release. Type species: P. parontospora. [Book ref. 73,
112113.]
planospore A motile SPORE.
plant viruses VIRUSes which can infect and replicate in plants.
(cf. VIROID; VIRUSOID.) Commonly, plant viruses show a low
degree of host specificity, and some can also replicate in insects.
Infection of a plant by a given virus may be systemic spreading
rapidly via the phloem (or occasionally xylem) or slowly from
cell to cell via plasmodesmata or may remain localized at the
site of infection. (Spread is apparently a virus-specific function
involving virus-encoded or virus-induced proteins [review: AVR
(1984) 29 313364].) Infection may be symptomless (silent,
latent), or may involve the development of symptoms ranging
from mild to severe or lethal; symptoms, when present, often
depend on the species and variety of the host plant, on the
particular virus strain, and on environmental conditions, and
may be affected by the presence of another virus or of a
Envelope
Nucleocapsid morphology
dsDNA
ssDNA
dsRNA
isometric
paired isometric particles
isometric
ssRNA
ssRNA
monopartite
rod-shaped
caulimoviruses
geminiviruses
plant reoviruses (Reoviridae), rice ragged stunt virus, some
cryptic viruses
plant rhabdoviruses (Rhabdoviridae), tomato spotted wilt virus
isometric
monopartite
rod-shaped or filamentous
bipartite
isometric
bipartite
tripartite
tripartite
multipartite
rod-shaped or filamentous
isometric
rod-shaped
filamentous
and
RHABDOVIRIDAE.
(cf.
plasmid
environment does not select for the genetic diversity needed
by species in more challenging environments [FEMS Reviews
(1998) 22 255275]; however, some intracellular bacteria (e.g.
Chlamydia spp) are known to contain plasmids [see e.g. Microbiology (1997) 143 18471854].
Many plasmids encode product(s) and/or functions(s) which
modify the phenotype of the host cell. Almost any feature may
be encoded by plasmids, including e.g. resistance to particular
ANTIBIOTIC(s) and/or HEAVY METAL(s) (see R PLASMID), and the
synthesis of AGROCINS, BACTERIOCINS, GAS VACUOLES (e.g. in
certain strains of Halobacterium), restriction endonucleases (see
also PHAGE TYPING), SIDEROPHORES, toxins (see e.g. ANTHRAX
TOXIN, ETEC) or virulence factors (see e.g. CROWN GALL and VW
ANTIGENS). Some plasmid-encoded products alter the antigenic
characteristics of a cell (see e.g. ANTIGEN GAIN), and some
confer the ability to utilize particular substrate(s) (see e.g.
LACTOSE PLASMID, OCT PLASMID, TOL PLASMID). One plasmid may
counteract the effects of another; for example, the pSa plasmid
can abolish the specific adherence properties of Agrobacterium
strains which are due to the presence of the Ti plasmid [JGM
(1983) 129 36573660]. (See also CRYPTIC PLASMID.)
The presence of a plasmid within a cell may often be inferred
from the cells phenotype: certain characteristics are commonly
plasmid-specified. Whether or not a plasmid is present may be
determined e.g. by gel ELECTROPHORESIS of a CLEARED LYSATE, or
by treating the cells with certain agents that eliminate plasmids
(see CURING sense 2) and observing for the loss of particular
phenotypic properties. [Plasmid technology: Book ref. 177.]
Some plasmids can promote their own intercellular transfer
by CONJUGATION (sense 1b): see CONJUGATIVE PLASMID; some
conjugative plasmids contain a TRANSFER OPERON which is
DEREPRESSED for conjugal transfer. (See also EPIDEMIC SPREAD.)
In addition to their own intercellular transfer, some conjugative
plasmids can mobilize the host cells chromosome (or certain
types of non-conjugative plasmid) for intercellular transfer (see
CONJUGATION sense 1b).
More than one type of plasmid can occur in a given cell;
plasmids which have different modes of replication (see below)
and of PARTITION are said to exhibit compatibility, i.e., they can
co-exist stably in the same cell. Plasmids which have similar
or identical replication/partition systems are incompatible, i.e.,
they cannot co-exist stably in the same cell; the phenomenon of
incompatibility enables plasmids to be classified into a number
of incompatibility groups (Inc groups): see INCOMPATIBILITY.
Plasmid replication. A plasmid controls its own replication,
using the cells biosynthetic machinery to make any plasmidencoded proteins etc. that are needed; plasmid DNA REPLICATION
requires various host proteins commonly e.g. the product of
the DNAB GENE, the DNAC GENE, the dnaE gene (D polC gene:
see DNA POLYMERASE) and the dnaG gene (see PRIMASE) in
Escherichia coli. (See also DNAA GENE.)
Replication is not coupled to any specific stage or event in
the CELL CYCLE, and in some plasmids it occurs throughout the
cell cycle.
Replication and PARTITION appear to be independent processes,
although both can determine INCOMPATIBILITY.
The rate-limiting step in replication is initiation, and the
rate of initiation is controlled in ways that differ according to
plasmid.
In some plasmids the control of initiation involves constitutive
synthesis of small, trans-acting ANTISENSE RNA molecules. Thus,
e.g. in plasmid ColE1 control involves the synthesis of two,
free (i.e. non-duplexed) strands of plasmid-encoded RNA, one
plasmid pInv
growth conditions. Such plasmids (e.g. ColE1) are said to be
under relaxed control; a typical relaxed plasmid is a small,
non-conjugative MULTICOPY PLASMID whose copy number under
normal conditions is ca. 1030. (A relaxed plasmid can exceed
its normal copy number only under abnormal conditions. See
also CLONING.) Plasmids which fail to replicate on inhibition of
protein synthesis are said to be under stringent control; a typical
stringent plasmid is a large, low-copy-number CONJUGATIVE
PLASMID.
Whether a plasmid is relaxed or stringent depends on its
system of replication control. Thus, e.g. in the relaxed COLE1
PLASMID (q.v.), not only is ongoing protein synthesis not required
for replication, but the inhibition of protein synthesis eliminates
a protein (Rom/Rop) which is inhibitory to plasmid replication.
Conversely, in stringent plasmids replication involves e.g. the
synthesis of proteins that are essential for the initiation of
replication.
[Control of plasmid replication: Book ref. 161, pp. 189214.]
Some plasmids have mechanisms for ensuring their persistence within a bacterial strain: see e.g. ccd mechanism in entry
F PLASMID.
Nomenclature. Plasmids are designated in various ways.
COLICIN PLASMIDS are designated according to the colicins
they encode (e.g. ColE1-K30 encodes colicin E1, ColV,I-K94
encodes colicins V and Ia). Many antibiotic-resistance plasmids
are designated by the letter R followed by a number, e.g. R1,
R46 etc; others include e.g. R6K, RK2, RP1 etc. Recombinant
plasmids are often indicated by the prefix p, e.g. pML31. A
number of plasmids are given trivial names (e.g., 1), while the
names of some indicate particular functions (see e.g. Ti plasmid
under CROWN GALL, and TOL PLASMID).
(See also entries for individual plasmids: e.g. COLE1 PLASMID;
DELTA; F PLASMID; PBR322; PMB1; PML31; PSC101; R1 PLASMID; R46
PLASMID; R100 PLASMID; R6K PLASMID; RP1 PLASMID.)
plasmid pInv See EIEC.
plasmid pYV See FOOD POISONING (Yersinia).
plasmin See FIBRINOLYSIN.
plasminogen (profibrinolysin) An inactive precursor of FIBRINOLYSIN normally present in blood; it is a large (90 kDa)
glycoprotein.
Plasminogen has been found to bind disease-associated PRIONS, but not the normal protein (PrPC ); this property may
be useful in diagnostic tests for TRANSMISSIBLE SPONGIFORM
ENCEPHALOPATHIES [Nature (2000) 408 479483].
plasmodesma (pl. plasmodesmata) A fine channel in a plant
cell wall or a fungal SEPTUM through which cytoplasm can
pass; plasmodesmata allow continuity between the cytoplasm
of adjacent cells. (See also DESMOTUBULE, PIT CONNECTION and
PLANT VIRUSES.)
plasmodiocarp See MYXOMYCETES.
Plasmodiophora See PLASMODIOPHOROMYCETES and CLUBROOT.
Plasmodiophorea See RHIZOPODA.
Plasmodiophorina See GYMNOMYXA.
Plasmodiophoromycetes (endoparasitic slime moulds) A class
of eukaryotic organisms (division MYXOMYCOTA) which are
obligate intracellular parasites in plants, algae and fungi. The
vegetative stage of the organisms is a plasmodium (a naked,
multinucleate protoplast); hyphae and fruiting bodies are apparently never formed. Although traditionally regarded as fungi,
the true taxonomic position of these organisms remains uncertain; they are apparently unrelated to other members of the
Myxomycota. rRNA data studies support the idea that they
may be at the base of an evolutionary line leading to the
of which, RNA II, can bind at the plasmids origin and act as a
primer, thus permitting replication. The other strand, RNA I, can
interfere by base-pairing with RNA II such that the outcome
of RNA IRNA II interaction determines the occurrence, or otherwise, of replication (for further details see COLE1 PLASMID). (It
appears that RNA I is normally polyadenylated, such polyadenylation facilitating its degradation; in Escherichia coli, mutations
in the pcnB gene, which encodes a poly(A)polymerase, result in
RNA I molecules that are stabilized through lack of polyadenylation the effect of which is to inhibit replication of ColE1, i.e.
to reduce its copy number.) Once initiated, replication in ColE1
proceeds as in the E. coli chromosome, although in this plasmid
replication occurs unidirectionally from the origin.
In the R1 PLASMID (q.v.), antisense RNA molecules bind to, and
inhibit translation of, the mRNA of the RepA protein which,
in turn, is involved in regulating the frequency of plasmid
replication.
Many of the small circular plasmids in Gram-positive bacteria
(and some in Gram-negative bacteria) replicate by a ROLLING
CIRCLE MECHANISM. Replication is initiated by a plasmid-encoded
Rep protein which, by nicking a specific strand at the origin,
generates a 30 end for synthesis. One round of replication
produces a complete dsDNA plasmid and a circular ssDNA
copy, the latter then being replicated to the dsDNA state from an
RNA primer. In some of these plasmids initiation is controlled
by regulation of the synthesis/activity of the Rep protein (as
the quantity of Rep protein affects the frequency of replication);
in some cases small, plasmid-encoded RNA molecules bind to
the rep mRNA and bring about either premature termination of
transcription or inhibition of translation. Alternatively, the Rep
protein may be inactivated after only one use by binding to a
small plasmid-encoded oligonucleotide. [Replication control in
rolling circle plasmids: TIM (1997) 5 440446.]
In many plasmids of Gram-negative bacteria, the Rep initiator
protein binds to direct repeats of nucleotides (iterons) in the
region of the plasmids origin of replication, thus contributing to
a nucleoprotein complex that initiates replication. For example,
in the F PLASMID, RepE (the E protein) carries out this function;
replication proceeds by a bidirectional Cairns-type mechanism
(as in the E. coli chromosome). (See also R6K PLASMID.) For
each plasmid, the iterons have a characteristic number, spacing
and composition. In some plasmids, Rep can also repress
transcription of its own gene by binding to inverted repeat
sequences overlapping the promoter; in some cases (including
the F plasmid) it has been shown that, while monomers of
Rep bind to iterons (promoting replication), dimers bind to
the promoters of their own genes (inhibiting replication). RepA
monomers (as opposed to dimers) of the Pseudomonas plasmid
pPS10 may be structurally suitable for RepAiteron binding
[EMBO (1998) 17 45114526].
In general, plasmid replication and PARTITIONing seem likely
to depend on some kind of association between the plasmid and
the cytoplasmic membrane [Mol. Microbiol. (1997) 23 110].
Under normal growth conditions, replication is initiated at
a frequency which, for a given plasmid in a given type of
cell under given conditions, leads to the establishment of a
characteristic COPY NUMBER. During steady-state conditions each
plasmid replicates, on average, once per cell division although
the inter-replication period may vary widely from one plasmid
to another.
If protein synthesis is inhibited (e.g. by CHLORAMPHENICOL),
some plasmids can continue to replicate, and can achieve
copy numbers much higher than those achieved under normal
594
Plasmodium
Chytridiomycetes, Ascomycotina and Basidiomycotina, but do
not exclude the possibility of a protozoal ancestry [TBMS
(1983) 80 107112]. (cf. RHIZOPODA and GYMNOMYXA.) Genera include Ligniera, Octomyxa, Plasmodiophora, Polymyxa,
Sorodiscus, Sorosphaera, Spongospora, Tetramyxa, Woronina.
(cf. ENDEMOSARCA; PHAGOMYXA.) Species are parasitic in e.g.
higher plants (e.g. Plasmodiophora brassicae in crucifers see
CLUBROOT; Spongospora subterranea in potatoes see POWDERY
SCAB; Ligniera betae in beet; L. junci in various monocots and
dicots); in algae (e.g. Woronina in Vaucheria, Sorodiscus in
Chara); and in certain aquatic fungi (e.g. Woronina in Achlya,
Pythium or Saprolegnia). Infected tissues often exhibit hypertrophy and sometimes hyperplasia.
In e.g. Plasmodiophora brassicae and Polymyxa betae, infection of a new host is initiated when a (primary) zoospore
attaches to the wall of a root hair, withdraws its flagella, and
encysts. Within the encysted cell there develops a tubular structure, the Rohr, containing an osmiophilic spine-like structure,
the Stachel. The Rohr evaginates rapidly, and the Stachel punctures the host cell wall; the protoplast of the encysted zoospore
then enters the host cell and develops into a vegetative primary
(D sporangiogenous) plasmodium. When mature, this plasmodium gives rise to uninucleate secondary zoospores, each with
two smooth flagella of different lengths. [Secondary zoospore
development in P. brassicae: TBMS (1984) 82 339342.] The
zoospores are released either by disintegration of the host cell
or via an exit tube arising from the zoosporangium. The role
of these zoospores in the life cycle is unclear; fusion between
two zoospores has been reported, but karyogamy when it
occurs is apparently delayed. A zoospore (or fused pair of
zoospores?) infects another host cell, in which it develops
to form a (diploid?) secondary (D cystogenous) plasmodium.
When mature, this plasmodium eventually cleaves to form
a number of uninucleate, thick-walled, resistant cysts (resting spores); meiosis has been observed at this stage in several species. [Ultrastructure of meiosis in Woronina pythii :
Mycol. (1984) 76 10751088.] In some species the cysts are
arranged in characteristic clusters (cystosori). [Fine structure
of the cystosorus in Spongospora subterranea: CJB (1985) 63
22782282.] On disintegration of the host cell the cysts are
liberated into the soil where they may remain viable for long
periods (e.g. years). On germination, each cyst gives rise to a
biflagellate (heterokont) zoospore which can infect another host,
thus initiating a new cycle.
Some members of the Plasmodiophoromycetes are important
as vectors of certain plant viruses: see e.g. BEET NECROTIC YELLOW VEIN VIRUS, SOIL-BORNE WHEAT MOSAIC VIRUS, POTYVIRUSES,
TOBAMOVIRUSES.
plasmodium A multinucleated, usually motile mass of protoplasm which is usually naked (i.e., bounded only by a plasma
membrane) and which is generally variable in size and form;
plasmodia are the main vegetative forms in e.g. members of the
ACARPOMYXEA, MYXOMYCETES (q.v. for types), MYXOSPOREA and
PLASMODIOPHOROMYCETES. (cf. PSEUDOPLASMODIUM.)
Plasmodium A genus of protozoa of the suborder HAEMOSPORORINA. The genus includes the common causal agents of MALARIA
in man: P. falciparum [genome: Nature (2002) 419 498511],
P. malariae (formerly P. rodhaini), P. ovale and P. vivax.
P. cynomolgi and P. knowlesi are parasitic in non-human primates; they occasionally cause malaria in man, and have been
widely used as models in research on human malaria. P. berghei
and P. yoelii (also spelt P. yoelli ) cause rodent malaria; they
have been used for testing antimalarial drugs.
plasmogamy
plasmogamy Coalescence of the cytoplasm of two or more cells;
in fertilization, plasmogamy is followed by KARYOGAMY.
Plasmopara A genus of fungi of the PERONOSPORALES; species
include P. viticola and P. halstedi, the causal agents of DOWNY
MILDEWS on grape and sunflower, respectively.
plasmotomy In certain multinucleate protozoa (e.g. Actinosphaera, Pelomyxa): an asexual reproductive process in which
fission results in the formation of two or more multinucleate
daughter cells, the nuclei of the parent cell being more or
less evenly distributed between them; nuclear and cytoplasmic
divisions appear to occur independently.
plastics (from bacteria) See BIOPOL.
plastid Any of various types of membrane-limited, typically
DNA-containing organelle which occur within the cells of plants
and algae but not in those of animals or prokaryotes. Examples:
AMYLOPLAST, CHLOROPLAST, CHROMOPLAST, ELAIOPLAST, ETIOPLAST and LEUKOPLAST. (See also PLASTOME.)
plastocyanin A copper-containing BLUE PROTEIN which acts as
an electron donor to photosystem I (see PHOTOSYNTHESIS). In
certain algae (e.g. Scenedesmus) plastocyanin can apparently
be replaced by a c-type cytochrome in the absence of copper. [Structure and function of plastocyanin: Book ref. 146,
pp. 1931.]
plastoglobuli Osmiophilic lipid globules in the stroma of a
CHLOROPLAST.
plastome The genetic complement of a PLASTID.
plastoquinone See QUINONES and PHOTOSYNTHESIS.
plate (1) A solid MEDIUM in a PETRI DISH prepared (using an
ASEPTIC TECHNIQUE) by pouring a sterile molten (AGAR- or
GELATIN-based) medium into a Petri dish to a depth of 35 mm
and allowing it to set. Freshly-poured plates to be used e.g.
for STREAKING should be left for 1020 min in a 37 C hot-air
incubator with the lid partly off so that the surface moisture can
evaporate; such drying before inoculation prevents unwanted
spreading of the inoculum in the surface film of moisture. (See
also SPREAD PLATE.) (2) A plate CULTURE. (3) (verb) To inoculate
a plate: see PLATING.
plate dilution test See DILUTION TEST.
platelet factor 4 (PF4) See CHEMOKINES.
platelets (thrombocytes) Flat, disc-like, membrane-bounded bodies (ca. 2.5 m diam.) which occur in mammalian blood (ca.
250000/mm3 in human blood); they are formed by fragmentation of megakaryocytes in red bone marrow. Platelets adhere to
rough or damaged surfaces and assist in blood clotting (though
clotting can occur in their absence). Platelets contain e.g. HISTAMINE and SEROTONIN.
plating (1) The act of distributing an INOCULUM on the surface
of a PLATE see e.g. SPREAD PLATE and STREAKING. (2) (serol.)
The use of specifically coated plastic (or other) surfaces for the
separation of specific cells (or other entities) from heterogeneous
populations. The procedure is based on antigenantibody specificity; thus, e.g., antibody, immobilized (by its Fc portion) on an
inert support, will bind, and thus remove from a mixture, those
cells which bear homologous cell-surface antigens.
Platyamoeba See AMOEBIDA.
Platymonas See TETRASELMIS.
plcB gene See LISTERIOSIS.
plectenchyma (mycol.) A tissue composed of hyphae or cells;
such tissues occur e.g. in LICHEN thalli, in fungal fruiting bodies,
etc. There are two principal types of plectenchyma: prosenchyma
(prosoplectenchyma), in which the hyphae remain distinguishable, are rather loosely woven, and are more or less parallel
to each other; and pseudoparenchyma (paraplectenchyma), in
Pleurastrum
597
plus-progamone
Diagnosis of Pneumocystis pneumonia typically involves
microscopy of induced sputum or of fluid from broncho-alveolar
lavage. Asci can be seen by staining with either TOLUIDINE
BLUE or Gomoris silver stain. Individual cells are detected
with Giemsa or Wrights stain [AJCP (1984) 81 511514].
Immunofluorescence stains are also available for P. carinii.
[Pneumocystis carinii (epidemiology, pneumonia, laboratory
diagnosis, therapy etc.): BCID (1995) 2 409576. Immune
response to P. carinii infection: TIM (1998) 6 7175. P. carinii
pneumonia in pigs (immunohistochemical study): VR (2000) 147
544549.]
pneumolysin See THIOL-ACTIVATED CYTOLYSINS.
pneumonia Inflammation of the lungs. It may involve the alveoli
(cf. ALVEOLITIS) and/or the interstitial tissues (interstitial pneumonia); inflammation may affect most of the parenchyma in one
or more lobes (lobar pneumonia) or may be diffuse. Pneumonia
is commonly due to bacterial infection, often secondary to e.g.
viral URTI (such as INFLUENZA) or other infection (e.g. MEASLES);
other causal agents include e.g. viruses (see also PNEUMOCYSTIS). The pathogen may gain access to the lungs by inhalation
or via the blood or lymph systems (see e.g. bubonic PLAGUE).
Conditions which predispose to pneumonia include chronic lung
disease, debilitating illness, immunosuppression, etc. Symptoms
of pneumonia generally include fever, chills, rigors, malaise,
dyspnoea and chest pain; cough may be initially dry, later productive of purulent, sometimes bloody sputum. Lab. diagnosis:
examination of sputum, pleural fluid etc by microscopy, culture, and/or serological techniques (e.g. CIE). Sputum may be
obtained by percutaneous aspiration from the trachea, rather than
by expectoration, to reduce contamination by members of the
normal respiratory tract flora.
(a) Pneumococcal pneumonia (classical lobar pneumonia),
caused by certain strains of Streptococcus pneumoniae (the
pneumococcus), is the commonest form of bacterial pneumonia. Infection may be primary or secondary. The pathogen,
present e.g. in the upper respiratory tract of carriers, gains access
to the lungs by inhalation. Incubation period: 13 days. Affected
lobes typically become consolidated, i.e., solidifed with inflammatory material (leucocytes, fibrin, pneumococci etc). Sputum
is initially purulent, becoming rusty or blood-stained as the
consolidation breaks down. Complications include e.g. pericarditis, meningitis etc. Chemotherapy: e.g penicillins, erythromycin.
Polyvalent vaccines containing polysaccharide antigens of various common pneumococcal serotypes are available for certain
high-risk patients [NEJM (1984) 310 651653; AIM (1986) 104
106109, 110112, 118120].
(b) Haemophilus influenzae (usually type b) may cause primary pneumonia (mainly in children) or secondary pneumonia in
patients with e.g. viral respiratory tract infection. The pneumonia
may be diffuse or lobar, and abscesses may develop. Chemotherapy: e.g. ampicillin; tetracycline; chloramphenicol.
(c) Staphylococcus aureus can cause lobar or diffuse interstitial pneumonia, usually following e.g. influenza or staphylococcal septicaemia. Abscesses may develop in lungs and/or
pleura. Sputum is yellow, purulent, and sometimes bloody. Proteases from some strains of S. aureus may activate influenza
virus virions (by cleaving their haemagglutinins: see INFLUENZAVIRUS), thus promoting combined viralbacterial pneumonia
[Nature (1987) 325 536537]. Chemotherapy: e.g. b-lactamaseresistant b-lactam antibiotics.
(d) Friedlanders pneumonia (caused by Klebsiella pneumoniae) is a severe form which usually occurs as a complication of
e.g. chronic lung disease. Typically, one or more lobes become
poky mutant
subsequently darken. [Phytopathol. Paper number 24 (March,
1981).]
Podaxales See GASTEROMYCETES.
podetium (lichenol.) A vertical, stem-like, lichenized structure
of generative tissue (sometimes called a secondary thallus)
which develops from a crustose, squamulose or foliose basal
(primary) thallus and which supports one or more hymenial
discs (apothecia); the entire podetium together with its
hymenial disc(s) should be regarded as a fruticose APOTHECIUM
[Lichenol. (1982) 14 105 113]. (cf. PSEUDOPODETIUM.) Podetia
are formed e.g. by most species of CLADONIA; they are usually
hollow and may be branched or unbranched or in some
Cladonia spp may terminate in a cup- or funnel-shaped
structure (the scyphus). (According to the above definition,
structures resembling podetia but lacking algae are not true
podetia; such structures are formed e.g. by Baeomyces spp and
Cladonia caespiticia.)
Podophrya See SUCTORIA.
podophyllotoxin A substance of plant origin (obtained from
Podophyllum peltatum) which has antitumour activity. Podophyllotoxin, which contains a trimethoxy-substituted aromatic ring,
binds to TUBULIN at a site close to (or identical with) that at
which COLCHICINE binds inhibiting the assembly of MICROTUBULES. Some epipodophyllotoxins (which have been used as
antitumour agents) appear to affect DNA synthesis (rather than
microtubule assembly) apparently by inhibiting topoisomerase
activity.
Podoscypha See APHYLLOPHORALES (Stereaceae).
Podosphaera See ERYSIPHALES.
Podospora A genus of fungi (order SORDARIALES) which occur
e.g. on soil and dung; the organisms form dark ascospores,
each bearing gelatinous appendages, in persistent asci formed
in perithecia. In P. anserina the four binucleate ascospores
per ascus each contain nuclei of compatible mating types (cf.
secondary HOMOTHALLISM). (See also AMIXIS.)
Podoviridae A family of DNA-containing BACTERIOPHAGES
which have isometric or elongated heads and short (ca. 20 nm)
non-contractile tails. Members include BACTERIOPHAGE N4, P22,
f29, T3, T7 (type species), and TBILISI PHAGE (see separate entries).
(See also MV-L3 PHAGE GROUP and SPIROPLASMAVIRUSES (SV-C3).)
Pogosta disease See SINDBIS VIRUS.
Poikilovirus See ALPHAHERPESVIRINAE.
point mutation (1) A type of MUTATION in which a single
nucleotide is replaced by another: see TRANSITION MUTATION
and TRANSVERSION MUTATION. A point mutation in a structural
gene may result in a MIS-SENSE MUTATION, a NONSENSE MUTATION,
or a SAME-SENSE MUTATION. Mutagens which can induce point
mutations include e.g. 5-BROMOURACIL, HYDROXYLAMINE and
NITROUS ACID.
(2) Any mutation involving a single nucleotide, including the
gain or loss of a nucleotide (resulting in a FRAMESHIFT MUTATION)
as well as transition and transversion mutations.
(cf. MULTISITE MUTATION.)
poising system See REDOX POTENTIAL.
Poitrasia See MUCORALES.
pokeweed mitogen (PWM) Any of five mitogenic LECTINS (designated Pa-1 to Pa-5) obtained from the roots, leaves and berries
of the pokeweed, Phytolacca americana. All can stimulate T
cells; Pa-1, in the presence of T cells and macrophages, can
stimulate Ig secretion by B cells. PWM binds to oligomers of
b-D-acetylglucosamine.
poky mutant A mutant strain of Neurospora which has a
subnormal rate of growth owing to a deficiency in its respiratory
pol genes
polaroplast See MICROSPORA.
polB gene See DNA POLYMERASE.
polC gene See DNA POLYMERASE.
poliomyelitis (polio; infantile paralysis) An acute infectious disease of humans, particularly children, caused by any of three
serotypes of human poliovirus (see ENTEROVIRUS). (A few nonhuman primates, e.g. chimpanzees, are also susceptible.) Transmission occurs by the faecaloral route (e.g. by person-toperson contact or via sewage-contaminated water). Incubation
period: 335 (usually 714) days. Infection may be asymptomatic; clinical forms are usually mild and self-limiting, with
fever, headache, nausea and vomiting, and pharyngitis (abortive
poliomyelitis). In a minority of cases the virus may invade the
CNS, causing inflammation and destruction of the lower motor
neurones in the brain stem and spinal cord. In non-paralytic
poliomyelitis symptoms include those of MENINGITIS (e.g. stiffness of the neck and back). In paralytic poliomyelitis there is
weakness and eventually flaccid paralysis of muscles (commonly
of the legs); the paralysis may or may not be permanent. Polio
is not usually fatal, but may be if respiratory muscles become
involved. Lab. diagnosis: serological tests; culture of the virus
from pharyngeal secretions and faeces. (See also SALK VACCINE
and SABIN VACCINE.)
polioviruses See ENTEROVIRUS.
Polish infectious dropsy (of carp) See CARP ERYTHRODERMATITIS.
pollen mould Bettsia alvei (q.v.).
pollution (environmental) See ENVIRONMENTAL POLLUTION.
poly(A) tail See MRNA.
polyacetylenes (polyynes) Linear compounds, containing both
double and triple bonds, which are produced by certain
higher fungi (particularly basidiomycetes) and which, in some
cases, exhibit antifungal and antibacterial activity; the polyacetylene molecule usually has an oxygen-containing terminal group (e.g. a carboxyl or hydroxyl group). For example,
mycorrhizal Leucopaxillus cerealis produces diatretyne nitrile
(HOOCCHDCHCCCCCN) which is active e.g.
against Phytophthora cinnamomi.
polyacrylamide gel electrophoresis ELECTROPHORESIS using a
polyacrylamide gel see e.g. SDS-PAGE.
polyadenylated mRNA See MRNA.
polyamines Polycationic compounds containing two or more
amino groups; they appear to occur in all animal, plant and
microbial cells and in certain viruses.
Putrescine [NH2 (CH2 )4 NH2 ], spermidine [NH2 (CH2 )3 NH
(CH2 )4 NH2 ] and spermine [NH2 (CH2 )3 NH(CH2 )4 NH(CH2 )3
NH2 ] appear to be almost universally present in prokaryotic and
eukaryotic microorganisms. However, their cellular location(s)
and biological function(s) are still not known, although
numerous effects on e.g. nucleic acid structure and enzyme
activity have been observed in vitro; polyamines may have a
role e.g. in protein synthesis in bacteria, and are necessary for
the replication of at least some bacteriophages, including the
T-even phages (which contain putrescine and spermidine) and
bacteriophage l. (See also BACTERIOPHAGE fW-14.)
Polyamines are synthesized primarily from amino acids e.g.
putrescine may be formed by the decarboxylation of ornithine
or by the combined action of arginine decarboxylase and
agmatine ureohydrolase. (See also DECARBOXYLASE TESTS.)
In bacteria the polyamine content is significantly affected
by the growth conditions. A number of novel polyamines
have been described from extreme thermophiles: e.g. Thermus thermophilus contains polyamines such as thermine
poly-b-hydroxybutyrate
and small molecules; the polyene molecule may form a pore in
the membrane through which such leakage may occur. These
antibiotics are microbistatic at low concentrations, microbicidal
at higher concentrations.
Macrolide polyenes are effective against yeasts and other
fungi and also against protozoa, but not against most bacteria
(whose membranes lack sterols cf. MYCOPLASMA).
The selective toxicity of the clinically useful macrolide
polyenes is apparently due, at least in part, to their greater
affinity for ergosterol (a principal sterol in fungal cytoplasmic
membranes) compared with cholesterol (the main sterol in
mammalian cell membranes) (cf. FILIPIN).
Macrolide polyenes include e.g. AMPHOTERICIN B; AUREOFUNGIN; CANDICIDIN B; ETRUSCOMYCIN; FILIPIN; HAMYCIN; NYSTATIN;
PERIMYCIN; PIMARICIN; and TRICHOMYCIN.
(b) A group of structurally novel polyenes (produced by
actinomycetes [FEMS (1984) 25 121124]) which are active
against prokaryotes, inhibiting PROTEIN SYNTHESIS. In bacteria, aurodox, azdimycin, dihydromocimycin, efrotomycin, factumycin, kirromycin (D mocimycin) and kirrothricin all act by
binding to EF-Tu and preventing its dissociation from the ribosome; the structurally related antibiotic pulvomycin binds EFTu-GTP and prevents the formation of the aa-tRNA-GTP-EF-Tu
complex, thus preventing the binding of aa-tRNA to the ribosomal A site. In archaeans, elongation factors are generally
insensitive to kirromycin, and the elongation factors of only
some archaeans are sensitive to pulvomycin [JB (1986) 167
265271].
polyether antibiotics See MACROTETRALIDES.
polyethylene glycol (PEG; Carbowax)
A polymer, H(OCH2 .
CH2 )n OH, available in a range of grades of mean MWt between
ca. 200 and ca. 20000; above MWt ca. 1000 it is a solid, below it
is a liquid. PEG is used e.g. in cell fusion (see e.g. HYBRIDOMA),
in PROTOPLAST FUSION, in artificial TRANSFORMATION systems, and
as a precipitating agent in clinical chemistry. PEG is also used for
concentrating, by osmosis, serum and other aqueous solutions
and suspensions; serum etc is placed in a U-shaped tube of
semipermeable material (e.g. Visking tubing) and the tubing partly
submerged in a concentrated aqueous solution of PEG.
poly(ethylene oxide) A high-MWt polymer (CH2 CH2 O)n
used e.g. to increase the viscosity of a medium in order to slow
down rapidly motile organisms see COUNTING METHODS. (cf.
FICOLL.)
polygenic mRNA See MRNA.
polyhedra (virol.) Large inclusion bodies formed in the cells
of insects infected with certain viruses (see CYTOPLASMIC POLYHEDROSIS VIRUS GROUP and BACULOVIRIDAE); a polyhedron is
composed of a matrix of crystalline, virus-specific protein (polyhedrin) in which mature virions are embedded (occluded).
Polyhedra are stable structures which appear to give some protection to the virions they contain; they serve as vehicles for
virus transmission: ingestion of polyhedra by a new host is followed by degradation of polyhedrin in the gut and the release of
infectious virions. Polyhedra can be isolated from infected cells
e.g. by differential centrifugation.
polyhedral bodies See CARBOXYSOMES.
polyhedrin See POLYHEDRA and BACULOVIRIDAE.
polyhedrosis An INSECT DISEASE caused by a NUCLEAR POLYHEDROSIS VIRUS or by a virus of the CYTOPLASMIC POLYHEDROSIS
VIRUS GROUP.
poly-b-hydroxyalkanoate See POLY-b-HYDROXYBUTYRATE.
poly-b-hydroxybutyrate (PHB) A linear polymer of b-hydroxybutyrate (D()-3-hydroxybutyrate): H-[O.CH(CH3 ).CH2 .CO]n OH. It occurs as refractile granules in the cells of various
Polyhymenophorea
which is synthesized by a multifunctional enzyme, polyketide
synthase. The possibility of developing new drugs by genetic
engineering of the polyketide synthetic pathway has been hindered by the difficulty of carrying out such work with actinomycetes; to address this problem, synthetic potential (including
polyketide synthase activity) has been incorporated into a strain
of Escherichia coli which can now synthesize the nucleus of
the erythromycin molecule [Science (2001) 291 17901792;
commentary: Science (2001) 291 1683].
polylinker A region of DNA containing close/overlapping sites
for different RESTRICTION ENDONUCLEASES. Synonym: multiple
cloning site (MCS).
polymerase chain reaction See PCR.
polymetaphosphate See POLYPHOSPHATE.
polymorph (polymorphonuclear leucocyte) (1) Syn. PMN. (2)
Syn. NEUTROPHIL.
polymorphic Refers to e.g. an organism which exhibits POLYMORPHISM.
polymorphism (1) The ability of an organism to occur in two or
more morphologically distinct forms (MORPHOTYPES), according
e.g. to conditions (as in PHAEODACTYLUM) or to the stage in the
life cycle (e.g. TRYPANOSOMATIDAE). (cf. PLEOMORPHISM sense 1).
(2) Syn. PLEOMORPHISM (sense 1).
(3) (in nucleic acids) A variant region of nucleotides in a
related nucleic acid molecule e.g. a variant sequence found in
a given allele in one or more strains of an organism but not in all
strains of that organism. Some authors use the term even when
the variation in sequence consists of only a point mutation.
Polymyxa See PLASMODIOPHOROMYCETES.
polymyxins A group of peptide ANTIBIOTICS produced by various
species of Bacillus (e.g. B. polymyxa); they include e.g. antibiotics formerly classified as circulins and colistins. Polymyxins
are active against many Gram-negative bacteria exceptions
including e.g. many strains of Neisseria and Proteus, and the
eltor biotype of Vibrio cholerae (the cholerae biotype is susceptible); most Gram-positive bacteria and most fungi are resistant, but some strains of e.g. Candida are susceptible. Against
bacteria, polymyxins are bactericidal to both growing and nongrowing cells.
Polymyxins have MWts of ca. 10001200, and they contain
a high proportion of a,g-diaminobutyric acid (DAB). The
polymyxin molecule is a cyclic heptapeptide with a peptide
side-chain that terminates in a fatty acid residue; the fatty acid
is 6-methyloctanoic acid in e.g. polymyxins A, B1, D1 and E1
(D colistin A), and is 6-methylheptanoic acid in e.g. polymyxins
B2, D2 and E2. Variations also occur in the constituents of
the cyclic and linear peptides. [Structure of polymyxins: Book
ref. 14, pp. 189194.]
In Gram-negative bacteria, polymyxins act by increasing the
permeability of the CYTOPLASMIC MEMBRANE to small molecules
and by damaging the OUTER MEMBRANE. Polymyxin B nonapeptide, a derivative of polymyxin B which lacks the fatty acid
residue, lacks the bactericidal activity of polymyxin B but is
able to damage the outer membrane [CJM (1986) 32 6669].
(See also OCTAPEPTINS.)
polynucleotide kinase An enzyme used e.g. for the 50 -end
labelling of a PROBE (q.v.).
polynucleotide phosphorylase (PNPase) An enzyme, present
e.g. in Escherichia coli and other prokaryotes, which in vitro
can catalyse e.g. the phosphorolysis of poly- or oligoribonucleotides in the presence of phosphate, and the polymerization
of ribonucleoside diphosphates.
polyol (polyhydric alcohol) Strictly: any compound containing
more than one alcohol group. As commonly used, the term refers
PROKARYOTES,
Polyporus
to a sugar alcohol, i.e., the compound obtained when the aldo
or keto group of a sugar is reduced to a hydroxy group. For
example, reduction of galactose gives galactitol (dulcitol), ribose
gives ribitol, etc. (cf. PLURONIC POLYOL F127.) [Polyol metabolism
in fungi: AMP (1984) 25 149193.] (See also e.g. PENTITOLS.)
polyoma virus (polyomavirus) (1) Mouse (murine) polyoma
virus: see POLYOMAVIRUS. (2) Any virus of the genus Polyomavirus (q.v.).
Polyomavirus A genus of viruses of the PAPOVAVIRIDAE. Type
species: mouse (murine) polyoma virus (polyoma virus); other
members include e.g. BK virus and JC virus (human viruses), K
virus (a mouse virus), SIMIAN VIRUS 40 (SV40), and stump-tailed
macaque virus (STMV). (See also BUDGERIGAR FLEDGLING DISEASE VIRUS.) Polyoma viruses can be propagated readily in suitable cell cultures (see e.g. SIMIAN VIRUS 40; cf. PAPILLOMAVIRUS).
The viruses generally appear to be common in their natural
hosts, in which infection is usually asymptomatic (although
JC virus which seems to be common in humans can cause
PROGRESSIVE MULTIFOCAL LEUKOENCEPHALOPATHY in certain circumstances); however, many polyoma viruses can be oncogenic
in other hosts: e.g. SV40, JC and BK can induce tumours in
newborn rodents and can transform several types of cell in culture. JC virus can also induce brain tumours in adult monkeys.
Cells transformed by SV40 or murine polyoma virus contain
viral DNA integrated into the host chromosomal DNA; integration occurs at non-specific sites and may involve the entire viral
genome or only a portion of it. However, integration appears not
to be essential for transformation by BK virus, and its significance in SV40 and polyoma virus transformation is unknown.
Expression of early viral genes appears to be necessary for transformation in all cases.
[Polyomaviruses and disease of the central nervous system:
RMM (1998) 9 7985.]
In murine polyoma virus, at least three distinct genes appear
to act in a coordinated manner to induce transformation in
primary rat embryo fibroblasts; the product of each gene induces
particular alterations in cell structure and growth control [Book
ref. 113, pp. 109116]. The three products are large T protein
or large T antigen (MWt ca. 105000), middle T protein or
middle T antigen (MWt ca. 56000), and small T (or t) protein
or small T antigen (MWt ca. 22000). The large T protein is a
DNA-binding protein which localizes in the host cell nucleus in
association with the chromatin. The middle T protein localizes
in the host cell plasma membrane; it is tightly associated with a
tyrosine-specific protein kinase identified as the c-src product
pp60c-src (see SRC [EMBO (1984) 3 585591]. The small T
protein is found in the soluble cytoplasmic fraction of the cell;
its activities are unknown, but it may disrupt actin cables in the
cell.
Viruses SV40, BK and JC appear to encode proteins corresponding to large T and small T proteins but do not encode a
middle T protein. In SV40, the large T antigen (T antigen)
is a multifunctional phosphoprotein MWt ca. 92000) which can
alone induce neoplastic transformation in cells from a variety
of species; it also acts as a key regulatory protein in the lytic
cycle of SV40 in permissive monkey cells. The protein binds
to SV40 DNA at multiple sites near the replication origin, has
ATPase activity, and binds to a host protein of MWt 53000. The
SV40 small T protein may also have a role in transformation; it
has been detected in the host cell cytoplasm and in the nucleus
[Book ref. 113, pp. 369375].
polyoxins A group of antifungal nucleosideoligopeptide antibiotics produced by Streptomyces cacaoi. Polyoxins are competitive inhibitors of chitin synthase, being structural analogues of
polyprotein
polyvalent antiserum Any antiserum which contains antibodies
to a number of different antigens.
polyvalent vaccine A single VACCINE containing the PROTECTIVE
ANTIGENS and/or toxoids from each of several different strains
of one species of pathogen. (cf. MIXED VACCINE.)
polyvinyl alcohol fixative A FIXATIVE: SCHAUDINNS FLUID with
five times the usual concentration of glacial acetic acid, supplemented with polyvinyl alcohol (5% w/v) and glycerol (1.5
ml per 100 ml fluid). Specimens can remain in PVA fixative,
without damage, for long periods of time.
polyvinyl pyrrolidoneiodine See IODINE (a).
polyynes Syn. POLYACETYLENES.
pomona fever LEPTOSPIROSIS caused by L. interrogans serotype
pomona.
Pontiac fever See LEGIONELLOSIS.
porcine circovirus (PCV) A small isometric virus (diam. 17 nm)
containing ccc ssDNA (MWt 0.58 106 ). PCV was isolated
from a porcine cell line, and is presumed to infect pigs
since specific antibodies to the virus were present in randomly
collected pig sera but not in the sera of other animals. PCV
apparently represents a new family of ANIMAL VIRUSES. [Nature
(1982) 295 6466.]
porcine haemagglutinating encephalitis virus See CORONAVIRUS
and VOMITING AND WASTING DISEASE.
porcine icteroanaemia See EPERYTHROZOONOSIS.
porcine parvovirus See PARVOVIRUS.
porcine reproductive and respiratory syndrome See BLUEEARED PIG DISEASE.
porcine transmissible gastroenteritis virus See CORONAVIRIDAE
and TRANSMISSIBLE GASTROENTERITIS.
pored epicortex (lichenol.) A polysaccharide layer (ca. 0.6 m
thick) which overlies the upper cortex in certain foliose lichen
thalli and which is perforated by numerous more or less regular
perforations ca. 1525 m or more in diameter. The underlying
cortex is continuous but is generally thin (e.g. 23 cell layers
thick), the cells being relatively loosely packed; these cortical
features, together with the pored epicortex, apparently allow
sufficient gas exchange to obviate the need for pseudocyphellae
or cyphellae [Lichenol. (1981) 13 110].
porfiromycin The N-methyl derivative of MITOMYCIN C.
Poria (1) A genus of lignicolous fungi of the APHYLLOPHORALES
(family Polyporaceae) which form resupinate fruiting bodies
(ranging from millimetres to centimetres in thickness) in which
the hymenophore is porous; the whitish context is monomitic and
lacks clamp connections. In perennial fruiting bodies the tubules
are stratified (cf. HETEROBASIDION). (See also BROWN ROT, COAL
BIODEGRADATION, DRY ROT, PACHYMAN and PAPER SPOILAGE.)
(2) Poria is sometimes used as a form genus to include those
polypores which form annual or perennial resupinate fruiting
bodies.
porin (formerly: matrix protein) In the OUTER MEMBRANE of
Gram-negative bacteria: a type of protein molecule which
usually in trimeric form (but sometimes dimeric or monomeric) forms a water-filled transmembrane channel (pore) that
permits the passage of certain ions and small molecules; porins
are also found e.g. in the mitochondrial outer membrane. (See
also LAMB PROTEIN and TSX PROTEIN.) Note that the term porin
is also used to refer to the complete pore structure whether it
be composed of one, two or three porin proteins.
Bacterial porins. Porins have been demonstrated in many
types of Gram-negative bacteria, but most studies have been
carried out on E. coli and Salmonella typhimurium. Although
porins are typically trimeric, dimeric porins have been found
porphyrins
glucose derivatives; a similar preference is shown by porin channels in Pseudomonas aeruginosa, but those in e.g. Neisseria
gonorrhoeae (and those in the mitochondrial outer membrane)
are preferentially permeable to anions. Negative charge may
make little difference (or enhance) the passage of a molecule
through the PhoE channel in E. coli. [Role of porins in outer
membrane permeability (review): JB (1987) 169 929933.]
Porin channels in LIPOSOMES can be opened and closed
by adjusting the value of the transmembrane potential; in
this way they resemble the voltage-controlled mitochondrial
porin channels (referred to as voltage-dependent anion channels VDACs). However, while the outer membrane can
exhibit a transmembrane potential under certain conditions, the
opening and closing of porin channels in intact cells has not been
shown to be regulated in this way. (See also LIPOSOME SWELLING
ASSAY.)
poroconidia See CONIDIUM.
porogenous development See CONIDIUM.
porospore See CONIDIUM.
porphin A cyclic TETRAPYRROLE in which the four pyrrole groups
are linked by their a-carbon atoms via methene (CHD)
bridges; porphin is the parent compound of the PORPHYRINS.
porphobilinogen A substituted monopyrrole: an intermediate in
the biosynthesis of PORPHYRINS.
Porphyra
A genus of marine algae (division RHODOPHYTA).
The nature of the thallus varies according to the stage in
the life cycle; the thallus can be sheet-like (one or two cells
thick) or filamentous the filamentous form being called the
Conchocelis stage since it was previously thought to be a
different organism (designated Conchocelis). The organisms,
which range from reddish-purple to olive green, attach to rocks
etc by means of a holdfast. (See also LAVER and PORPHYRAN.)
porphyran A group of complex, mucilaginous, sulphated and
methylated galactans (containing D- and L-galactose and 3,6anhydro-L-galactose) produced by Porphyra spp.
Porphyridium A genus of unicellular, spherical algae (division
RHODOPHYTA) which occur e.g. in freshwater habitats and on soil.
Each cell contains a stellate chloroplast with a central pyrenoid;
there is no cell wall, each cell being surrounded by a gelatinous polysaccharide capsule. When viewed in masses, the cells
may be blood-red (e.g. P. purpureum formerly P. cruentum)
to blue-green (e.g. P. aerugineum), depending on the relative
proportions of phycoerythrin and phycocyanin which they contain.
porphyrin test A test for determining the X FACTOR requirement
of a Haemophilus strain by determining the ability of the
strain to convert d-aminolaevulinic acid (ALA) to porphyrins
or porphobilinogen. A medium (0.5-ml aliquot) containing
ALA (2 mM) and MgSO4 (0.8 mM) in phosphate buffer (0.1 M,
pH 6.9) is inoculated with a loopful of bacteria from an agar
plate culture and incubated for ca. 4 hours at 37 C. A red
fluorescence from the culture (or culture fluid) under WOODS
LAMP (360 nm) indicates the formation of porphyrins (a positive
test, i.e., the strain does not require the X factor); alternatively,
0.5 ml Kovacs indole reagent may be added, shaken vigorously,
and the phases allowed to separate a red coloration in the lower
(aqueous) phase indicating the formation of porphobilinogen (a
positive test). [Book ref. 22, pp. 561562.]
porphyrins PORPHIN derivatives in which the pyrrole bcarbons are variously substituted: e.g., aetioporphyrins (D
etioporphyrins) have 4 methyl and 4 ethyl substituents,
mesoporphyrins have 4 methyl, 2 ethyl and 2 propionic acid
substituents, and protoporphyrins have 4 methyl, 2 vinyl and
port
2 propionic acid substituents. Isomers of a given porphyrin
are usually denoted by Roman numerals: e.g. aetioporphyrin
I is 1,3,5,7-tetramethyl-2,4,6,8-tetraethylporphin, and aetioporphyrin III is 1,3,5,8-tetramethyl-2,4,6,7-tetraethylporphin.
Protoporphyrin IX (D protoporphyrin III) is 1,3,5,8-tetramethyl2,4-divinylporphin-6,7-dipropionic acid. (The numbering system
used in the Dictionary illustrated in the figure for CHLOROPHYLLS is the widely used Fischer system; alternative systems
have been proposed in which, e.g., all carbon atoms in the
tetrapyrrole ring are numbered sequentially, 120, starting with
the a-carbon of ring I next to the d-methene position [PAC
(1979) 51 22512304].)
Porphyrins can readily chelate various metals, the metalloporphyrins being components of several important biological
pigments: see e.g. CHLOROPHYLLS, CYTOCHROMES, HAEM. (See
also CHLORIN; cf. PHYCOBILIPROTEINS.)
port See WINE-MAKING.
Port Salut cheese See CHEESE-MAKING.
porter See PERMEASE.
positive control (of an operon) See OPERON.
positive interference See INTERFERENCE (2).
positive-sense genome See VIRUS.
positive staining See ELECTRON MICROSCOPY (a).
positive-strand virus A VIRUS (q.v.) with a positive-sense
genome.
post-antibiotic effect (PAE) The suppression of bacterial growth
(typically for hours) which follows a short exposure to
some types of antimicrobial agent e.g. aminoglycosides, 4quinolones, b-lactams, streptogramins and macrolides. PAE is
a factor when considering the dose/dosage frequency of these
antibiotics; it can be advantageous when coincident with low
concentrations of an intermittently administered drug. PAE may
involve different mechanisms in different organismantibiotic
combinations [AAC (1995) 39 13141319].
The post-antibiotic sub-MIC effect may be more relevant,
clinically, than the PAE [JAC (1999) 43 7177].
post-ciliary microtubules (ciliate protozool.) A ribbon of MICROTUBULES which arises from the right-hand posterior side of
a kinetosome (close to triplet 9, GRAIN CONVENTION), extends
upwards (towards the pellicle) and to the right, and then (sometimes) runs posteriorly between the kineties, the wider face of
the ribbon being perpendicular to the body surface. (See also
PITELKA CONVENTION.)
posterior station (parasitol.) The hindgut and/or rectum of an
arthropod vector; infective forms of parasites in the posterior
station can be transmitted to the vertebrate host via the faeces
of the vector (see e.g. CHAGAS DISEASE). (cf. CONTAMINATIVE
INFECTION.)
post-fixation See FIXATION.
post-herpetic neuralgia See HERPES ZOSTER.
post-kala-azar dermal leishmaniasis A cutaneous leishmaniasis
which may occur in a patient up to two years after that
patient has been cured of VISCERAL LEISHMANIASIS. [PCR-based
diagnosis of post-kala-azar dermal leishmaniasis: JCM (1998)
36 16211624.]
post-meiotic segregation The segregation of alleles during the
first nuclear division after MEIOSIS; it results from the separation
of strands of uncorrected heteroduplex DNA (in a chromatid)
formed previously during recombinational events in meiosis (see
RECOMBINATION).
`
606
Powassan encephalitis
mosaic virus, carnation vein mottle virus, carrot thin leaf virus,
celery mosaic virus, cocksfoot streak virus, cowpea aphid-borne
mosaic virus (of which Azuki bean mosaic virus is a strain),
leek yellow stripe virus, lettuce mosaic virus, onion yellow dwarf
virus, Papaya ringspot virus, parsnip mosaic virus, peanut mottle
virus, PLUM POX virus, potato virus A, soybean mosaic virus,
sugarcane mosaic virus (of which maize dwarf mosaic virus is
a strain), tobacco etch virus, tulip breaking virus, turnip mosaic
virus.
Many other viruses have been tentatively included as possible
members of the potyviruses. These include (a) certain aphidborne viruses: e.g. carrot mosaic virus, celery yellow mosaic
virus, groundnut eyespot virus, tobacco vein mottling virus,
tomato (Peru) mosaic virus, wheat spindle streak virus, wheat
streak virus; (b) a group of viruses which are transmitted by
eriophyid mites: e.g., Agropyron mosaic virus, oat necrotic
mottle virus, ryegrass mosaic virus, Spartina mottle virus, wheat
streak mosaic virus; (c) the whitefly-transmitted virus sweet
potato mild mottle virus; and (d) a group of viruses transmitted
by Polymyxa graminis: barley yellow mosaic virus, oat mosaic
virus, rice necrosis mosaic virus, wheat spindle streak mosaic
virus, wheat yellow mosaic virus. Some or all of these possible
members may actually belong to or constitute separate groups.
pouch (food processing) See RETORT POUCH.
poultry diseases Poultry (chickens, ducks, turkeys, etc) can be
affected by a wide range of diseases some specific for one
species of bird, others affecting a range of birds. (a) Bacterial
diseases: see e.g. AIR SACCULITIS; ARIZONOSIS; BUMBLEFOOT;
COLISEPTICAEMIA; DIPHTHEROID STOMATITIS; erysipelas (see
powdery mildews
VIRUS).
Pribnow box
prephenate See AROMATIC AMINO ACID BIOSYNTHESIS.
preprimosome See PRIMOSOME.
pre-protein See SIGNAL HYPOTHESIS.
pre-reduced medium See ANAEROBE.
preservation (1) (of materials, products) The use of physical
and/or chemical means to kill or prevent the growth of those
microorganisms which, by their growth and/or activities, may
cause BIODETERIORATION of a given material or product. Physical methods (e.g. heat STERILIZATION, freezing see e.g. FOOD
PRESERVATION) either kill contaminating organisms or render the
materials or products unsuitable for the (rapid) growth of likely
contaminants. Chemical agents (PRESERVATIVES) may be microbistatic or microbicidal.
(2) (of microorganisms) Viable populations of microorganisms
may be preserved (i.e. maintained for reference purposes etc)
by e.g. FREEZING, FREEZE-DRYING or DESICCATION. Some bacterial
cultures can be preserved by sealing with a layer of sterile
mineral oil and storing at ca. 4 C. A culture may be preserved
by periodic SUBCULTURE (see also STABILATE).
preservative Any chemical used for the PRESERVATION of materials or products; in some industries such chemicals are referred
to as BIOCIDES. For examples of preservatives and their usage
see e.g. FOOD PRESERVATION, PAINT SPOILAGE, PAPER SPOILAGE,
SAUSAGE, TEXTILE SPOILAGE, TIMBER PRESERVATION; see also ALCOHOLS, BISPHENOLS, CHLORBUTANOL, EGME, FORMALDEHYDE, GERMALL 115, PHENOLS, QUATERNARY AMMONIUM COMPOUNDS, SALICYLANILIDES, THIOMERSAL. A preservative may be inactivated
e.g. by colloids (such as magnesium trisilicate or bentonite cf.
BENZOIC ACID; CHLORBUTANOL) or by certain container materials
(polyethylene can inactivate e.g. dichlorophenol and other phenolics, while polypropylene can inactivate e.g. dichlorophenol
and sorbic acid).
prespore See ENDOSPORE (sense 1(a)).
pressure-cycle fermenter See AIRLIFT FERMENTER.
presumptive coliform count See COLIFORM TEST.
pretibial fever Syn. FORT BRAGG FEVER.
pretrichocyst See TRICHOCYST.
pretyrosine See AROMATIC AMINO ACID BIOSYNTHESIS.
Prevotella A genus of Gram-negative, asporogenous, anaerobic,
rod-shaped bacteria found e.g. in the human oral cavity; some
species form black or brown pigments when grown on bloodcontaining media. Most species ferment sucrose and lactose.
Using quantitative culture on a non-selective blood-agar
medium, studies on the anaerobic oral microflora in the first year
of life found that organisms in the Prevotella melaninogenica
group were among the early colonizers (18% at 2 months, rising
to 57% at 6 months and 77% at 12 months); members of the
P. intermedia group were apparently late colonizers, whereas
isolation of non-pigmented species of Prevotella increased from
occasional at 2 months to 75% at 12 months [RMM (1997) 8
(supplement 1) S19S20].
Species of Prevotella have been associated with e.g. abscesses
and PERIODONTITIS. [Simultaneous detection of Prevotella intermedia and Bacteroides forsythus by multiplex PCR in clinical
samples: JCM (1999) 37 16211624.]
pre-zygotic exclusion During processes such as CONJUGATION
(sense 1b) and TRANSDUCTION: the absence of expression of a
given donor gene in the recipient as a result of the failure of
that gene to enter the recipient. If the gene entered the recipient
but failed to recombine with the recipients genome, the absence
of expression of that gene is referred to as post-zygotic exclusion.
prgI gene (Salmonella typhimurium) See NEEDLE COMPLEX.
Pribnow box See PROMOTER.
PrausnitzKustner
test (PK test) A test used for demonstrat
ing the presence of IgE antibodies homologous to a given
allergen. Serum from a hypersensitive subject is injected intradermally into a normal subject; subsequent injection of the normal subject with the given allergen causes a WHEAL-AND-FLARE
response to develop within minutes (a positive test). The PK
reaction can be inhibited by the prior injection of a fragment of
e-chain [Nature (1985) 315 577578].
PRD See CATABOLITE REPRESSION.
PRD1 phage group Syn. TECTIVIRIDAE.
preaxostyle See OXYMONADIDA.
pre-B cell See B LYMPHOCYTE.
prebiotic (1) A non-digestible part of a food (often an oligosaccharide) which, by selectively stimulating certain type(s) of
colon bacteria, benefits the host.
(2) (adj.) The time before life appeared on Earth.
prebuccal area In some ciliates (e.g. Paramecium): a depression
in the body surface leading to the BUCCAL CAVITY; its ciliature is
essentially somatic (cf. VESTIBULUM).
precipitation (serol.) The formation of a precipitate when antibodies and soluble antigens react in suitable proportions (see e.g.
OPTIMAL PROPORTIONS; cf. ANTIGEN EXCESS and AGGLUTINATION).
(See also GEL DIFFUSION.)
precipitin An ANTIBODY which forms a precipitate with its
homologous soluble antigen. (cf. AGGLUTININ.)
precipitin test Any serological test in which the interaction of
antibodies with soluble antigens is detected by the formation of
a precipitate.
precipitinogen (1) An antigen which elicits a PRECIPITIN. (2) Any
agent (e.g. PROTEIN A) which can combine with antibody to form
a precipitate.
precyst See CYST (a).
prednisone See IMMUNOSUPPRESSION.
pre-erythrocytic schizogony (in Plasmodium) See PLASMODIUM.
pre-filtration See FILTRATION.
pre-fixation See FIXATION.
pre-genome See HEPADNAVIRIDAE.
pregnancy test An IMMUNOASSAY in which urine is examined for
human chorionic gonadotrophin (hCG), a hormone that appears
during pregnancy. Urine is added to serum containing antihCG antibodies, which combine with hCG. Then, the absence
of uncombined antibodies (a positive test) is shown by nonagglutination when latex-bound hCG is added.
pre-initiation complex See PROMOTER.
PreiszNocard bacillus See CORYNEBACTERIUM.
pre-lesion terminus In damaged DNA: the nucleotide immediately 50 of the lesion site.
premunition (concomitant immunity; non-sterilizing immunity)
(immunol.) Protective immunity, in respect of a given
pathogen, due to the persistence of small numbers of that
pathogen in the host; the host can resist superinfection (i.e.,
infection by the same or closely related pathogens) but cannot
achieve STERILIZING IMMUNITY. In an apparently analogous
phenomenon, cells of a given tumour type fail to develop when
injected into an animal suffering from the same type of tumour.
`
Pril
primate T-cell leukaemia virus See SIMIAN T-CELL LEUKAEMIA
VIRUS.
prime plasmid A PLASMID which has undergone aberrant excision from a bacterial chromosome. In some types of prime
plasmid (type I), part of the plasmid has been left behind in
the chromosome, and the plasmid carries a sequence of bacterial
DNA; a type II prime plasmid consists of the entire plasmid
carrying a sequence of bacterial DNA. The particular sequence
of bacterial DNA carried by a prime plasmid depends on the site
within the chromosome occupied by the plasmid before excision;
thus, e.g. it is possible to isolate various F0 plasmids (derived
from the F PLASMID) because this plasmid can integrate at various
sites in the bacterial chromosome.
(See also specialized TRANSDUCTION.)
primed (immunol.) (1) (of persons, animals) Refers to those
individuals who have had an initial immunological contact with a
given antigen; such individuals may respond e.g. with ANTIBODY
FORMATION. Subsequent exposure of a primed individual to
the given antigen may bring about a heightened response (see
ANAMNESTIC RESPONSE and HYPERSENSITIVITY (sense 1)). (See also
IMMUNE RESPONSE.) (2) (of cells) Refers to those cells whose
responsiveness to a given antigen has been heightened as a
consequence of their previous contact with that antigen (or of
previous contact between their precursor cells and that antigen).
(cf. PRIMING.)
primer See (i) DNA REPLICATION; (ii) PCR; (iii) NASBA; (iv) SDA;
and (v) FORWARD PRIMER.
primer-dimer In a PCR reaction mixture: an artefact resulting
from the use of a pair of primers whose 30 terminal sequences are
mutually complementary; during extension, each primer uses the
other as a template forming products that consist essentially
of two double-stranded primers in tandem.
priming (1) (mol. biol.) The initiation of synthesis of a DNA
strand e.g. by the synthesis of an RNA primer (see DNA
REPLICATION). (For specific and general priming see DNAB
GENE.)
(2) (immunol.) The process in which an individual becomes
PRIMED.
primite The anterior organism of a pair of gregarines in SYZYGY.
(cf. SATELLITE.)
primociliatid gymnostomes Presumptively primitive ciliates
(subclass GYMNOSTOMATIA, order Primociliatida) which are
homokaryotic; species of STEPHANOPOGON are the only known
examples.
primordium (microbiol.) Syn. INITIAL(s).
primosome A multiprotein complex involved in certain cases of
primer synthesis (see DNA REPLICATION): e.g. in BACTERIOPHAGE
fX174 DNA synthesis, and in Okazaki fragment synthesis during
Escherichia coli chromosome replication and e.g. COLE1 PLASMID
replication. Primosome formation on ssDNA coated with SINGLESTRAND BINDING PROTEIN is initiated by protein n0 (D factor Y)
which recognizes and binds to specific short base sequences in
the DNA. In the presence of ATP, a complex of DnaB (see
DNAB GENE) and DnaC proteins is formed which, together with
proteins i (D factor X), n, and n00 combine with n0 to form
a prepriming intermediate (preprimosome) at or near the n0
recognition site. The preprimosome is recognized and bound by
the DnaG protein (PRIMASE) to complete the primosome. The
primosome migrates along the ssDNA template in a 50 -to-30
(anti-elongation) direction (i.e., in the direction of replication
fork movement in dsDNA replication), driven by ssDNAdependent ATP hydrolysis by n0 , and primase synthesizes short
RNA primers at many different sites on the template DNA. The
probe
others use superscripts which indicate the specific disease (e.g.
GSS for GerstmannStrausslerScheinker syndrome).
[Protein misfolding in prion disease: Cell (1997) 89 499510;
human prion diseases: Book ref. 215, pp. 3977.]
(2) Strains of the yeast Saccharomyces cerevisiae contain a
protein release factor (see PROTEIN SYNTHESIS) designated eRF3
(D Sup35, product of gene SUP35 ) which, through variation in
its effective concentration in the cytoplasm, can influence the
fidelity with which translation is terminated on the ribosome;
thus, a lowered concentration of the release factor promotes
readthrough at certain stop codons. A non-genetic mechanism
which can control the concentration of eRF3 may therefore
permit heritable variation in the organism without changes in
the genome [see e.g. Nature (2000) 407 477483].
Sup35 can exist in an aggregated, prion form (the [PSIC ] state)
or in a soluble form (the [psi ] state). In [PSIC ] cells, aggregation
of Sup35 protein reduces the amount available for terminating
translation on the ribosomes, and this allows readthrough at
certain stop codons.
Propagation of [PSIC ] involves proteinprotein interaction
following the mixing of cytoplasm from different cells (e.g.
during mating); in this process the soluble form of Sup35 is
converted to the aggregated (prion) form. (Interestingly, if a
[PSIC ] strain of S. cerevisiae is grown in the presence of 2 M
glycerol (or certain other agents) the aggregates of Sup35 break
down to the soluble form of Sup35, i.e. a [psi ] strain of the yeast
is formed.) [Elimination of [PSIC ] by guanidine hydrochloride:
Mol. Microbiol. (2001) 40 13571369.]
[eRF3 concentration in the termination of translation: Microbiology (2001) 147 255269 (262263).]
In vitro studies involving fusion between the prion domain
of Sup35 proteins from S. cerevisiae and Candida albicans may
help to explain factor(s) which determine the ability of a prion
to cross a species barrier [Nature (2001) 410 223227].
pristane An isoprenoid alkane: 2,6,10,14-tetramethylpentadecane.
pristinamycins See STREPTOGRAMINS.
pRNA See BACTERIOPHAGE f29.
PRNP gene See PRION.
probasidium (1) A developing BASIDIUM at the stage at which
karyogamy occurs; in many basidiomycetes the terms probasidium and METABASIDIUM refer to the same structure at different
developmental stages.
(2) That part of a developing basidium in which karyogamy
occurs e.g. the teliospore (or its contents) of the rust and smut
fungi, or, in Septobasidium, the typically thick-walled structure
from which arises, by outgrowth, the septate, basidiosporebearing metabasidium.
probe A short strand of DNA or RNA (often 1025 nucleotides
in length) which is complementary to a given target sequence of
nucleotides; because a probe can hybridize specifically with its
target sequence, it can be used e.g. to detect, identify or locate
the target. To make the probe detectable it is labelled either
before or after it hybridizes to the target sequence (see below).
(In addition to DNA or RNA, probes may also be prepared from
PNA [JAM (2001) 90 180189].)
Probetarget hybridization is affected e.g. by temperature,
pH and concentration of electrolyte. Conditions can be chosen such that the probe will hybridize only to the exact target
sequence, i.e. conditions under which mis-matches are not tolerated; such high-stringency conditions are used to promote
specificity in probetarget binding. Under low-stringency conditions the effect of mis-matched base(s) can be minimized so
probenecid
that hybridization may occur even when the probetarget duplex
contains mis-matched base(s).
The detection of RNA targets may be achieved with greater
rapidity and specificity by means of 20 -O-methyl oligoribonucleotide probes (compared with 20 -deoxy oligoribonucleotide
probes) [NAR (1998) 26 22242229].
Labelling of probes. Probes may be labelled directly and
covalently with radioactive isotopes (e.g. 32 P); such isotopic
labels can be detected by autoradiography. Both DNA and RNA
probes can be labelled at the 50 end with e.g. [g32 P]ATP (i.e.
ATP with 32 P in the g position); this reaction is mediated by
polynucleotide kinase. Radioactive labels are robust, and are
associated with good sensitivity (but limited resolution).
Non-radioactive (non-isotopic) labelling with e.g. enzymes
or fluorescent molecules is common. Labelling may be either
direct or indirect. Thus, for example, existing probes may be
labelled with a reactive fluorophore which binds covalently
to the probe; such labelling systems are available commercially (e.g. FluoReporter , marketed by Molecular Probes Inc.,
Eugene, OR, USA). In the second form of direct fluorescent
labelling, probes are synthesized in a reaction mixture containing fluorophore-conjugated nucleotides (which are thus incorporated into the probe). Such fluorescent nucleotides are available
commercially (e.g. ChromaTide ; Molecular Probes Inc.). Fluorescent labels are detected by examining the preparation under
ultraviolet light.
CHEMILUMINESCENCE is used in probe detection in certain
commercial diagnostic tests (see e.g. hybridization protection
assay in the entry TMA).
Note that, in direct labelling, the probe is already labelled
prior to hybridization.
For indirect labelling (e.g. with an enzyme or fluorophore), a
small molecule (e.g. a biotin or DIGOXIGENIN tag) is incorporated into the probe before use. After hybridization, the probe is
detected by using a conjugate to link the tag with a fluorophore
or enzyme see e.g. DOT-BLOT. (It has been reported that short
(10-nucleotide) 50 -biotinylated probes give satisfactory results
when labelled with a STREPTAVIDIN alkaline phosphatase conjugate prior to the hybridization step [NAR (1999) 27 703705].)
Uses of probes. Probes can be used e.g. to detect, identify
or locate particular pathogens in clinical specimens (by demonstrating the presence of pathogen-specific sequences); specimens
are commonly subjected to pre-test procedures in which any
target nucleic acids that may be present are exposed (in singlestranded form) to specific probes. One example is the PACE 2C
test (Gen-Probe, San Diego, USA) which, in a single assay, can
detect Chlamydia trachomatis and/or Neisseria gonorrhoea in
urogenital specimens [see e.g. JCM (1995) 33 25872591].
In situ hybridization (ISH) involves the use of strain- or
species-specific probes e.g. for detecting pathogens in situ i.e.
at the actual site of infection within tissues or cells; bacterial,
viral, fungal and protozoal pathogens may be detected. ISH
is particularly useful for demonstrating nucleic acids which
are focally distributed e.g. virus-infected tissue. For example,
ISH was found to be as sensitive as PCR for the detection
of human papillomavirus in cervical scrapings [HJ (1995) 27
5459]. Much of the early work in ISH was conducted with
radioactive probes; currently, fluorescent probes are common
(fluorescence in situ hybridization: FISH). FISH is both rapid
and flexible. For example, the target area can be interrogated
simultaneously with several different types of probe (each
labelled with a different fluorophore); thus, when different
probes bind to closely adjacent targets they can be distinguished
by their emission characteristics.
promoter
progressive pneumonia virus See LENTIVIRINAE.
proguanil See CHLORGUANIDE.
prohead A DNA-free phage head precursor formed during
bacteriophage assembly. (See e.g. BACTERIOPHAGE T4; see also
SCAFFOLDING PROTEIN.)
prohormone See PHEROMONE.
prokaryote (procaryote) A type of CELLULAR (sense 2 or 3)
MICROORGANISM in which the CHROMOSOME(s) are not separated
from the cytoplasm by a specialized membrane; the CYTOPLASMIC
MEMBRANE is typically devoid of sterols; chloroplasts and
mitochondria are absent (cf. INTRACYTOPLASMIC MEMBRANES);
RIBOSOMES have a sedimentation coefficient of ca. 70S; a CELL
WALL is typically present and may contain structural components
such as PEPTIDOGLYCAN or PSEUDOMUREIN, or may consist e.g.
of an S LAYER; storage compounds may include e.g. POLYb-HYDROXYBUTYRATE; flagella (when present) are structurally
relatively simple (see FLAGELLUM (a) and (c)).
CHEMOLITHOAUTOTROPHS, and the ability to carry out NITROGEN
FIXATION, occur only among the prokaryotes.
The prokaryotes comprise two DOMAINS: the domain ARCHAEA
(formerly referred to as the kingdom Archaebacteria) and the
domain BACTERIA [JB (1994) 176 16]. Members of the two
domains differ in their 16S rRNA and e.g. in the composition,
structure and/or mode of assembly of the cytoplasmic membrane, cell wall and flagella; differences also occur e.g. in the
composition of the ribosomal proteins.
According to one hypothesis, EUKARYOTES arose from an
energy-based symbiotic relationship between cells from the two
prokaryotic domains [Nature (1998) 392 3741].
prolamellar body In an ETIOPLAST: a paracrystalline array of
tubules bearing a small lamellar structure (prothylakoid ) which
contains certain thylakoid components (e.g. the CF1 unit of
PROTON ATPASE); on illumination, prolamellar bodies disperse,
and prothylakoids eventually develop into THYLAKOIDS.
prolate Of a phage head: having a shape in which the distance
from one pole to the other is greater than the diameter at the
mid-point of the head; an example of a prolate head occurs in
BACTERIOPHAGE f29.
proliferative kidney disease (PKD) A FISH DISEASE which can
be economically important in young salmonid fish. Symptoms
include exophthalmia, anaemia, abdominal swelling and kidney
hypertrophy; mortality rate: 1095%. PKD is caused by an
unclassified protozoon which apparently has affinities with
members of the MYXOZOA [JP (1985) 32 254260].
Proliferobasidium See BRACHYBASIDIALES.
L-proline biosynthesis See Appendix IV(a).
proloculus See FORAMINIFERIDA.
promastigote A form assumed by the cells of many species of
the TRYPANOSOMATIDAE (q.v.) during at least certain stages of
their life cycles.
prometaphase See MITOSIS.
Promicromonospora A genus of asporogenous bacteria (order
ACTINOMYCETALES, wall type VI) which occur e.g. in soil. The
organisms form a yellow fragmenting mycelium. GC%: ca. 73.
Type species: P. citrea. [Book ref. 73, pp. 5354.]
promiscuous plasmids Those CONJUGATIVE PLASMIDS (sense
1) e.g. IncP1 plasmids which are capable of self-transmission
between bacteria of a wide range of different species and genera.
promitochondrion See MITOCHONDRION.
promoter In a DNA strand: a nucleotide sequence which is
recognized (directly or indirectly) and bound by a DNAdependent RNA POLYMERASE (RPase) during the initiation of
TRANSCRIPTION. Transcription is initiated at a position (the start
promoter control
point or start site) which is commonly within the promoter
sequence. The first nucleotide to be transcribed is designated
C1; nucleotides downstream of this position (i.e. those in the
direction of RNA elongation: 50 -to-30 with respect to the RNA)
are numbered C2, C3, C4 etc., and nucleotides in the opposite
(upstream) direction are numbered 1, 2, 3 etc.
Bacteria have several RPase holoenzymes (differing in their
SIGMA FACTORS), each one recognizing a distinct class of promoter. In Escherichia coli most transcription is carried out by
Es70 ; the enzyme binds to a region of DNA extending from
ca. 50 bp upstream to ca. 20 bp downstream of the start point.
Comparison of the sequences of many promoters recognized by
Es70 has revealed that certain short sequences are more or less
conserved. Thus, a CONSENSUS SEQUENCE, TATAAT (the Pribnow
box or 10 sequence), is centred ca. 10 bp upstream from the
start point, and another consensus sequence, TTGACA (the 35
sequence) is centred ca. 35 bp upstream of the start point. The
start point itself is usually a purine, often an adenine residue in
the sequence CAT.
Promoters recognized by Es70 in E. coli differ to varying
extents from the theoretical consensus promoter, and may also
differ from one another in functional efficiency (efficient promoters being described as strong, inefficient ones as weak).
Efficiency may be affected e.g. by changes in the consensus
sequences or in the transcribed region downstream of the start
point. Changes at one site may be compensated for by changes
at another: thus, promoters with the same efficiencies may have
different base sequencies; furthermore, a (synthetic) promoter
containing the theoretical consensus sequences has been found
to be relatively inefficient.
Bacterial promoters of other classes (recognized by different
RPase holoenzymes) also typically have two short, distinctive
conserved sequences upstream from the start point; however, the
actual sequences vary from one class of promoter to another.
For example, in Bacillus subtilis the main holoenzyme, Es43 ,
recognizes the same type of promoter as does the Es70 of E. coli,
but Es37 (see SIGMA FACTOR) recognizes a consensus sequence
AGGATTTNA (N D any nucleotide) in the 35 region and
GGAATTNTTT in the 10 region; the corresponding sequences
for Es29 are TTNAAA and CATATT. (The phage T4 Esgp55
recognizes a promoter which apparently lacks a 35 sequence;
in promoters recognized by the EsgpntrA of e.g. Klebsiella a 35
sequence is apparently absent, but there is a consensus sequence
in the 20 region.)
In eukaryotes, promoters are not recognized directly by the
RNA polymerases; transcription initiation factors (TIFs) first
bind to a promoter to form a pre-initiation complex, and only
then does an RPase bind to form an initiation complex. Promoters for RPase II generally contain a short consensus sequence,
TATA(A/T)A(A/T) (the TATA box, GoldbergHogness box, or
Hogness box ), ca. 2530 bp upstream from the transcription
start point; this appears to be the only well-conserved sequence
in RPase II promoters [NAR (1986) 14 1000910026], although
other sequences upstream of the TATA box may be important
sites for the action of promoter-specific TIFs [review: Nature
(1985) 316 774778]. (See also ENHANCER.)
The TATA box, found in many RPase II promoters, also occurs
in a minority of type III promoters. The classical RPase III
promoters occur within the associated gene, i.e. intragenically,
downstream of the start point; binding of the RPase at the
promoter leads to initiation of transcription at a particular
distance upstream of the binding site.
One factor, the TATA box-binding protein (TBP), is necessary
for the formation of an initiation complex by each of the three
prostaglandins
OXIDE).
prostheca
the addition of microbial proteases to domestic detergents for the
digestion of proteinaceous stains in fabrics. Since most commercial detergents contain tripolyphosphate as a sequestering agent,
Ca2C -requiring proteases (e.g. THERMOLYSIN) are not suitable
for this purpose, and alkaline serine proteases (see SUBTILISINS)
from Bacillus spp are usually used. Enzymes from Rhizomucor
pusillus, R. miehei and Endothia parasitica have some use as
rennin (rennet) substitutes in CHEESE-MAKING (see also CASEIN);
the proteolytic-to-coagulating activity ratio of these enzymes is
higher than that of rennin, and their use requires some modification of the cheese-making process in order to avoid the
excessive formation of bitter peptides. Microbial proteases have
some application in the manufacture of leather, although chemical methods are still cheaper; alkaline proteases from alkalophilic
Bacillus spp may be used with lime for de-hairing hides, and
proteases from e.g. Aspergillus oryzae or Bacillus spp may be
used for bating hides (a process which makes the leather softer
and more elastic). Other uses include e.g. treatment of flour to
adjust its gluten composition (and hence baking qualities); as
a digestive aid; and in the debridement of wounds (experimental) and dissolution of blood clots (see e.g. BRINASE). (See also
PRONASE.)
Proteases produced by certain pathogenic microorganisms
may act as virulence factors (see e.g. ELASTASE).
proteasome A hollow, intracellular proteolytic structure formed
by the self-assembly (autocompartmentalization) of proteases
and ATPases; proteolytic sites occur in the interior of the
proteasome so that protein degradation can be carried out
intracellularly without risk to the cells integrity. A narrow
entrance to the proteasomes interior restricts access to unfolded
proteins.
In eukaryotes, proteasomes are used for the ATP-dependent
degradation of various UBIQUITIN-bound proteins. For example,
the ubiquitinproteasome pathway is reported to be essential during changes in morphology (e.g. trypomastigote !
amastigote) in Trypanosoma cruzi [Biochem. (2001) 40 1053
1062].
Proteasomes also occur in prokaryotes e.g. the archaeans
Methanosarcina thermophila and Thermoplasma acidophilum,
and the bacteria Mycobacterium tuberculosis and Rhodococcus
erythropolis.
[Proteasomes in prokaryotes: TIM (1999) 7 8892.]
(See also DEGRADOSOME.)
protectant (prophylactic) (plant pathol.) Any chemical agent
which prevents the occurrence of particular disease(s) among
plants treated with that agent. (cf. ERADICANT.)
protective antigens Those antigens of a pathogen which can
elicit an immune response that gives protective immunity against
the pathogen.
protective immunity Syn. IMMUNITY (3).
Proteeae A tribe of bacteria (family ENTEROBACTERIACEAE)
divided (e.g. on the basis of DNA relatedness) into three genera: MORGANELLA, PROTEUS and PROVIDENCIA. All members can
oxidatively deaminate a range of amino acids. Most strains are
motile (but may be non-motile at temperatures >30 C), urease Cve (cf. PROVIDENCIA), lactose ve (although some strains
may contain a Lac plasmid), indole Cve (cf. PROTEUS), VP
ve, MR Cve. Acid ( gas) is produced from glucose, and
a reddish-brown pigment is produced on nutrient agar containing 5% tryptophan. Species are generally resistant to bacitracin,
polymyxins and erythromycin. [Book ref. 46, pp. 12041224.]
protein 2 A PORIN of Escherichia coli.
protein A (SpA) A cell wall protein (MWt ca. 42000) found in
most strains of Staphylococcus aureus; it is covalently bound
protein synthesis
the EspB and EspE proteins of enteropathogenic E. coli (EPEC);
and the various Yops of Yersinia [the Yersinia Yop virulon: Mol.
Microbiol. (1997) 23 861867].
[Type III secretion systems (review): TIM (1997) 5 148156.]
Type IV systems are mechanistically distinct and not fully
understood; the following is an outline of a current model. In
these systems the secreted protein is synthesized as part of a
larger protein that consists of (i) an N-terminal signal peptide,
(ii) an a domain, and (iii) a C-terminal b domain. Initially, the
whole protein is translocated across the CM in a sec-dependent
manner, with cleavage of the N-terminal signal peptide. To
pass through the outer membrane, the b domain is believed to
form a b-barrel pore in the membrane through which the a
(passenger) domain is translocated.
At the bacterial surface, the a domain may (i) remain attached
(exposed to the environment); (ii) undergo cleavage, but remain
(non-covalently) attached; (iii) undergo cleavage and release
to the environment. Cleavage may be autocatalytic, or it may
involve another outer membrane protein such as the SopA
protease of Shigella or the OmpT protease of Escherichia coli.
In a type IV system, the translated protein (i.e. N-terminal C
a domain C b domain) has been termed an autotransporter.
(This term has also been used by some authors to refer
specifically to the b domain; other authors have used the term
to refer specifically to the a domain.)
Proteins transported by type IV systems include the (cellsurface-retained) IcsA protein, associated with Shigella invasiveness in dysentery; the IGA1 PROTEASES of Haemophilus influenzae,
Neisseria gonorrhoeae and N. meningitidis; and the AIDA-I system of Escherichia coli. The latter system has been used for
AUTODISPLAY.
Type V systems. These include the mechanism by which TDNA is transferred from Agrobacterium tumefaciens to the host
cell in CROWN GALL, and the secretion of pertussis toxin by
Bordetella pertussis.
Note on the designation of type IV and type V systems. The
name type IV secretion system has been widely used for autotransporters by a number of authors [see e.g. TIM (1998) 6
370378; Book ref. 218 (1999), p 42; Book ref. 223 (1999),
p 94]. Some authors [see Inf. Immun. (2001) 69 12311243]
have suggested that (i) autotransporters be called type V systems, and that (ii) secretory mechanisms referred to above as
type V systems be called type IV systems. In this dictionary the
designation type IV has been retained for autotransporters.
protein synthesis A protein consists essentially of one or more
polypeptides a polypeptide being a chain of amino acids linked
by peptide bonds (CO.NH). Polypeptides are folded into a
three-dimensional structure that is stabilized mainly by hydrogen
and/or disulphide bonds formed between amino acids in different
parts of the chain; the specific three-dimensional structure of a
given protein is associated with its biological role.
The biosynthesis of a protein is a complex process in which
the composition of the protein (i.e. the number, nature and
sequence of its amino acids) is decoded from information
contained in specific sequence(s) of nucleotides. In the majority
of organisms (including all cells), proteins are encoded by DNA;
in certain viruses, proteins are encoded by RNA. The information
in nucleic acids is expressed via a GENETIC CODE (q.v.).
Unlike the polymerization of nucleotides (see e.g. DNA SYNTHESIS), polypeptide chains are not synthesized by the polymerization of amino acids on a template. In fact, protein synthesis
occurs in several stages.
In all cases (in both prokaryotic and eukaryotic cells) the first
stage is the synthesis of an RNA copy of the particular DNA
the targeting pathway of Escherichia coli pre-secretory and integral membrane proteins is specified by the hydrophobicity of the
targeting signal [PNAS (2001) 98 34713476].
The second stage of the GSP, translocation across the OUTER
MEMBRANE, depends on a number of specific secretion factors.
Although the GEP occurs in E. coli, this organism apparently
does not secrete proteins via the GSP, i.e. it does not carry
out the second stage of the GSP. However, other species of
the Enterobacteriaceae do secrete proteins via this pathway. For
example, Klebsiella oxytoca secretes a lipoprotein enzyme, pullulanase (see DEBRANCHING ENZYME), whose translocation across
the outer membrane requires the products of 14 pul genes. (Interestingly, if all the pul genes from K. oxytoca are expressed in
E. coli, this organism can secrete pullulanase.) Again, the GSP is
used by Erwinia chrysanthemi for secreting the enzymes pectinase and cellulase, secretion needing expression of the out genes.
(E. coli encoding a gene for pectinase can secrete this enzyme
if supplied with out genes.) The secretory systems in K. oxytoca
and E. chrysanthemi are similar though not identical: K. oxytoca
can synthesize but not secrete a pectinase encoded by a gene
from E. chrysanthemi. (See also SECRETON.)
Pseudomonas aeruginosa secretes an exotoxin, and the
enzymes elastase and alkaline phosphatase, via a secretory system involving the xcp genes. Interestingly, XcpA is identical to
the PilD protein (involved in the formation of fimbriae) and is
also homologous to PulO, a protein involved in the secretion
of pullulanase, and it has been suggested that, in at least some
cases, the second phase of the GSP may involve a protein complex similar to the fimbrial assembly apparatus [TIG (1992) 8
317322; see also EMBO (2000) 19 22212228].
Folded proteins may cross the CM via the pmf-dependent Tat
system [see Microbiology (2003) 149 547556].
Type III systems. Secretion by type III systems occurs as a onestep process via a channel/pore which crosses the cell envelope
from cytoplasm to cell surface; unlike type I systems, the type
III pathway may involve 20 or more distinct proteins. (See also
NEEDLE COMPLEX.) Type III systems occur in certain pathogens
(including pathogens of plants [JB (1997) 179 56555662]).
(See also VIRULON.) [Type III secretory systems and pathogenicity islands (review): JMM (2001) 50 116126.]
Components of type III systems in various species exhibit
homology. Moreover, some type III components exhibit homology with components of other secretory systems e.g. components of the basal body of the (bacterial) FLAGELLUM.
Proteins secreted via type III systems include an N-terminal
sequence which may be targeted to the pore or channel but
which it is not cleaved.
The energy requirements of these systems are unknown, but a
pore-associated protein (YscN) in a type III system of Yersinia
includes binding sites typical of ATPases.
In some type III systems, protein secretion seems to be
activated by contact with a eukaryotic cell; at least some proteins
are believed to be secreted directly into the eukaryotic cytoplasm
because e.g. (i) proteins of the kind secreted by type III systems
typically have little or no effect on eukaryotic cells in the absence
of the secreting bacterium; (ii) some secreted proteins have been
detected within eukaryotic cells; and (iii) some proteins (Yops)
secreted by Yersinia have been associated with specific effects
within eukaryotic cells (see VIRULON). In EHEC and EPEC
strains of Escherichia coli, type III systems are reported to be
regulated by QUORUM SENSING (q.v.).
Proteins secreted by type III systems include e.g. the IpaB
protein of Shigella (which promotes APOPTOSIS in macrophages);
618
protein synthesis
sequence that encodes the given protein (see TRANSCRIPTION); as
this RNA transcript carries the genetic message from DNA it
is called messenger RNA (or, more usually, mRNA) see MRNA.
In some cases (commonly in eukaryotes, less commonly
in prokaryotes) the initial transcript must be processed to
remove non-coding part(s) (called introns) from the nucleotide
sequence see SPLIT GENE; the resulting (mature) mRNA is then
used to guide assembly of the polypeptide chain the stage of
protein synthesis called translation. mRNAs which lack introns
can be used directly for translation. (See also RNA EDITING.)
Along the length of the mRNA molecule, groups of three
consecutive bases each encode a particular amino acid. Each of
these three-base groups is called a codon; thus, e.g. the codon
UCA (uracil-cytosine-adenine) encodes the amino acid serine
(see table in GENETIC CODE). Hence, the sequence of codons in
mRNA encodes the sequence of amino acids in a polypeptide.
For the synthesis of a polypeptide, each amino acid must first
bind to a small adaptor molecule of RNA which is specific
for that amino acid and which also has a binding site (a threebase anticodon) for the appropriate codon. These RNA adaptor
molecules are called transfer RNA (tRNA) see TRNA. The
binding of a given amino acid to its tRNA (i.e. the charging of
a tRNA molecule) occurs in a two-step reaction. First, the amino
acid reacts with ATP in the presence of a specific aminoacyltRNA synthetase (forming an enzyme-bound aminoacyl-AMP
complex); the aminoacyl group is then transferred to the 20 or
30 position of the terminal adenosine residue in the tRNA (with
release of AMP and synthetase). (See also MUPIROCIN.)
The synthesis of a polypeptide on mRNA (i.e. the translation process) takes place on a RIBOSOME. In prokaryotes, correct
positioning of mRNA on the ribosome is facilitated by a particular sequence of nucleotides in the mRNA (the ShineDalgarno
sequence) located upstream of the coding region; this sequence
base-pairs with part of a 16S rRNA molecule in the 30S subunit
of the ribosome.
Essentially, following mRNAribosome binding, the ribosome moves along the mRNA molecule in such a way that each
codon, in turn, binds the relevant tRNA, and each successive
amino acid is linked, covalently, to the previous one.
The following outlines a generally accepted scenario for
protein synthesis in Escherichia coli; some details of the process
are still unknown. The process appears to be essentially similar
in most or all other bacteria.
Translation is initiated when mRNA binds to the ribosome.
Each ribosome has two (adjacent) binding sites for charged
tRNA molecules: the A site (D acceptor or entry site) and the
P site (D peptidyl or donor site). At the start of translation, the
first codon of mRNA (the initiator codon) coincides with the P
site. The initiator codon is usually AUG, but is sometimes e.g.
GUG, UUG or AUU.
The initiator codon is recognized by a distinct initiator tRNA
(tRNAi ) which is charged with methionine (Met). In E. coli there
are two tRNAs specific for methionine: tRNAm and tRNAf ; only
tRNAf can function as tRNAi (tRNAm being used for incorporation of Met in subsequent location(s) in the polypeptide
chain). In the charged tRNAf the a-amino group of the methionyl
residue is formylated (via N 10 -formyltetrahydrofolate), giving
fMet-tRNAf ; hence, the first (N-terminal) amino acid to be incorporated in the polypeptide chain is N-formylmethionine. (The
incorporation of N-formylmethionine as N-terminal amino acid
is typical of prokaryotes and of mitochondria and chloroplasts;
in the eukaryotic cytoplasm, and in at least some archaeans,
the methionine residue is not formylated, so that the N-terminal
amino acid in these cases is methionine.)
protein synthesis
for references], described for E. coli and e.g. Halobacterium
halobium, tRNAs remain bound to the ribosome both before
and after translocation, i.e. deacylated tRNA is not released from
the P site during translocation; instead, it is transferred to a
third ribosomal site (the E site) concomitantly with translocation. Release of deacylated tRNA from the E site is triggered by
the entry into the A site of the next (incoming) aminoacyl-tRNA.
Base-pairing between mRNA codons and tRNA anticodons
is not sufficiently stable, in itself, to guarantee the degree
of accuracy and efficiency needed in translation. It has been
suggested that proof-reading may occur e.g. at the level of amino
acid selection by aminoacyl-tRNA synthetases; when synthetase
specificity is not high enough to prevent binding of the wrong
amino acid, the latter may be recognized and removed either
at the aminoacyl-AMP stage (pre-transfer proof-reading) or at
the aminoacyl-tRNA stage (post-transfer proof-reading) [see e.g.
NAR (1986) 14 75297539]. Proof-reading may also occur
during elongation; aminoglycosides such as STREPTOMYCIN may
exert their effect on translational accuracy by interfering with
this proof-reading system. The ribosome itself may provide help,
and this appears to be given by the rRNA [see e.g. Nature (1994)
370 597598].
Termination of translation (i.e. cessation of polypeptide synthesis) occurs when a specific termination codon (UAA, UAG
or UGA in E. coli see GENETIC CODE) appears at the A site.
These codons are recognized by protein release factors (RFs);
RF-1 recognizes UAA and UAG, while RF-2 recognizes UAA
and UGA. The recognition of a termination codon by an RF is
followed by hydrolysis of the ester bond between the tRNA (at
the P site) and the polypeptide chain it carries thus releasing
the completed polypeptide; hydrolysis is catalysed by peptidyltransferase. A third factor, RF-3 (D S protein), may stimulate
the activities of RF-1 and RF-2.
Although the stop signal is traditionally regarded as a triplet
of bases (e.g. UAA), there is evidence that the base following a
stop codon influences the efficiency of termination, and it may
be that the actual stop signal is a four-base (or even longer)
sequence [Mol. Microbiol. (1996) 21 213219]. In E. coli the
efficiency of termination at a stop codon is also influenced by the
50 (upstream) nucleotide context of the codon, the mechanism
involving the C-terminal amino acid residues in the nascent
polypeptide. [Translation termination and stop codon recognition
(review): Microbiology (2001) 147 255269.]
As one ribosome translocates along the mRNA another can
fill the vacated initiation site and start translation of another
molecule of the polypeptide; thus, a given mRNA molecule
may carry a number of ribosomes along its length forming
a polyribosome or polysome. (A single ribosome is sometimes
called a monosome.)
At some time after the start of elongation, the formyl group of
formylmethionine (see earlier) or formylmethionine itself is
excised from the polypeptide. In E. coli, formylmethionine is
cleaved from about 50% of proteins; whether or not cleavage
occurs in a given protein appears to depend on the identity of
the penultimate N-terminal amino acid residue the longer the
side-chain on this residue the smaller the probability of cleavage
of formylmethionine. When such cleavage does occur it is
effected by METHIONINE AMINOPEPTIDASE (q.v.). When the formyl
group (only) is cleaved, the reaction is catalysed by methionine
deformylase (D peptide deformylase, PDF). (PDF is inhibited
by certain derivatives of hydroxamic acid, but these compounds
are unlikely to be useful as broad-spectrum antibacterial agents
because (i) they were bacteriostatic in the organisms tested, and
(ii) resistance develops readily [AAC (2001) 45 10581064].)
proton ATPase
P. morganii. See MORGANELLA.
P. myxofaciens. Indole ve; maltose Cve; ornithine decarboxylase ve; abundant slime produced e.g. in trypticasesoy
broth.
P. rettgeri. See PROVIDENCIA.
P. shigelloides. See PLESIOMONAS.
P. vulgaris. Indole Cve; maltose Cve; ornithine decarboxylase ve.
P. mirabilis and P. vulgaris occur e.g. in soil, polluted water,
intestines of (healthy) man and animals, etc. P. mirabilis, in
particular, is an important opportunist pathogen, causing nosocomial URINARY TRACT INFECTION, pneumonia, septicaemia, etc.
P. myxofaciens was isolated from gypsy moth larvae (Porthetria
dispar ).
[Book ref. 22, pp. 491494.]
prothallus (lichenol.) (1) Syn. HYPOTHALLUS (sense 1). (2) A
lichen thallus in the initial stages of development.
prothylakoid See PROLAMELLAR BODY.
proticins BACTERIOCINS from Proteus spp.
protist A member of the PROTISTA.
Protista (1) A taxon (kingdom) which includes the ALGAE,
FUNGI and PROTOZOA (collectively, the eukaryotic protists), and
the PROKARYOTES. (2) A KINGDOM comprising the eukaryotic
protists see (1) above. (cf. MONERA.)
protoaecidium See UREDINIOMYCETES stage I.
protoaecium See UREDINIOMYCETES stage I.
Protococcidiorida An order of protozoa of the subclass COCCIDIASINA.
Protococcus See PLEUROCOCCUS.
protocooperation In a mixed population of microorganisms: an
interaction between two (or more) different microorganisms
in which each organism benefits from the activities of the
other (e.g. each organism may produce a substance which
stimulates the growth of the other), but in which the interaction
is not obligatory for either organism. (See e.g. YOGHURT; cf.
MUTUALISM.)
protofilament See MICROTUBULES.
Protogonyaulax tamarensis Syn. Gonyaulax tamarensis.
protohaem See HAEM.
protokaryote Archaic term for PROKARYOTE.
protokerogen See KEROGEN.
protomerite In a cephaline gregarine: the anterior of the two
main regions of the (septate) cell (cf. DEUTOMERITE). In the late
trophozoite stage the anterior part of the protomerite may bear
an EPIMERITE.
protometer In a cell: a hypothetical sensor which can respond
to changes in proton motive force.
protomite See TOMITE.
Protomonas A genus of methylotrophic bacteria; the organisms
have been re-classified in the genus Methylobacterium [IJSB
(1985) 35 209].
proton ATPase (proton-translocating ATPase; HC -ATPase) Any
ATPASE which can couple ATP hydrolysis to the energydependent translocation of protons across an ENERGYTRANSDUCING MEMBRANE (see CHEMIOSMOSIS) and/or which can
catalyse the pmf-dependent phosphorylation of ADP to ATP. (cf.
PROTON PPASE.)
The most-studied HC -ATPases are the (F0 F1 )-type HC ATPases (also referred to as (F1 F0 )-type HC -ATPases) which
occur e.g. in the bacterial cytoplasmic membrane, in the mitochondrial (inner) membrane, and in the thylakoid membranes of
chloroplasts; these enzymes have a MWt of ca. 500000. Bacterial
(F0 F1 )-type HC -ATPases consist of two distinct parts: (a) the
proton circuit
F0 moiety, a hydrophobic protein (typically containing three
kinds of subunit designated a, b and c in Escherichia coli )
embedded in the membrane bilayer, and (b) the F1 moiety, a
hydrophilic protein (typically consisting of five kinds of subunit)
which has ATPase activity, and which projects like a knob on
a short stalk from the cytoplasmic face of the membrane.
(Some authors regard the projecting stalked knob as an artefact
[JUR (1985) 93 138143].) The knob of F1 consists of two
types of subunit (designated a and b), and the stalk consists of
three types of subunit (g, d and e). Mitochondrial (F0 F1 )-type
HC -ATPases are essentially similar in structure but are somewhat more complex; the stalk region of the enzyme complex
includes an OLIGOMYCIN-sensitivity-conferring protein (OSCP),
which does not occur in bacterial or chloroplast ATPases, and
a protein (called inhibitor protein, I, or IF1 ) which inhibits
the hydrolysis of newly-made ATP. The mitochondrial, bacterial and chloroplast ATPases all contain, in the F0 moiety, a
DCCD-binding protein which confers sensitivity to DCCD.
Nomenclature of HC -ATPases. HC -ATP-ases from different
sources are designated as follows: CF0 F1 (from chloroplasts);
EF0 F1 (from Escherichia coli ); MF0 F1 (from mitochondria);
TF0 F1 (from certain thermophilic bacteria, e.g. PS3). Individual components may be designated e.g. CF0 , EF1 , MF0 etc. The
three types of subunit in TF0 may be referred to as bands 4, 6
and 8 (from the SDSgel electrophoresis pattern). Other types of
HC -ATPase include the (E1 E2 )-type enzymes which occur e.g.
in the cytoplasmic membrane in certain fungi; these enzymes differ from (F0 F1 )-type ATPases e.g. in that their activity involves
the formation of a phosphorylated intermediate. (See also ATPASE
for a general note on the nomenclature of ATPases.)
ATP synthesis and hydrolysis. HC -ATPase-catalysed ATP synthesis requires a minimum pmf of ca. 100200 mV. During
ATP synthesis protons flow through the enzyme system, passing down the proton concentration gradient; the actual route
of proton flow appears to include the side-chains of particular
amino acids e.g. aspartic acid, glutamine, lysine and tyrosine.
(Interestingly, it has been proposed that the proton-conducting
pathway through another energy-transducing system, the purple
membrane (see BACTERIORHODOPSIN), involves a similar range
of amino acids.) Much or most of the energy derived from proton translocation may be used to effect the release of ATP from
the tightly cohesive ATPHC -ATPase complex rather than to
carry out the phosphorylation step itself. In one model it is
proposed that protons passing through the F1 moiety cause conformational changes in the enzyme which decrease the affinity
of ATP for the catalytic site. This type of model is believed to be
compatible with variable HC /P ratios the number of protons
needed to cause a given conformational change (with concomitant release of ATP) being postulated to vary with the prevailing
pmf.
Under some conditions HC -ATPases may catalyse either the
synthesis or hydrolysis of ATP in order that GATP and pmf
be more or less balanced (see CHEMIOSMOSIS). However, when
pmf is below a certain level, HC -ATPases are rapidly (and
reversibly) inactivated; such inactivation prevents depletion of
ATP e.g. under those conditions in which, for any reason,
the membrane is temporarily de-energized. In chloroplasts and
bacteria inactivation of HC -ATPases occurs as a result of the
tight binding between ADP and the catalytic site, while in
mitochondria the enzyme is inactivated by the inhibitor protein.
[Regulation of HC -ATPase activity: TIBS (1986) 11 3235.]
Inhibitors of (F0 F1 )-type HC -ATPases include e.g. AUROVERTINS, CITREOVIRIDIN, DCCD, EFRAPEPTIN, OLIGOMYCIN, QUERCETIN
Providencia
cell. Species occur e.g. in soil and water, and some can behave
as opportunist pathogens (see PROTOTHECOSIS).
protothecosis A disease, which affects man and animals, caused
by a species of Prototheca (commonly P. zopfii ); typically, it
involves the formation of localized skin lesions which may
be nodular, ulcerating and papular, or (rarely) granulomatous.
(See also MASTITIS.) A severe, often fatal, systemic form of the
disease also occurs, particularly in animals.
prototroph A strain of microorganism whose nutritional requirements do not exceed those of the corresponding wild-type strain.
(cf. AUXOTROPH.)
prototunicate ascus An ASCUS whose wall consists of a thin,
delicate membrane; the ascospores are released when the ascus
wall ruptures or deliquesces. Such asci are formed e.g. by
ascogenous yeasts.
protoxin A precursor form of a TOXIN: see e.g. DELTA-ENDOTOXIN.
protozoa A diverse group of eukaryotic, typically unicellular
microorganisms; they are classified as a subkingdom (Protozoa)
within the kingdom Animalia or the kingdom PROTISTA. (Some
of these organisms e.g. the SLIME MOULDS and members
of the PHYTOMASTIGOPHOREA are also classified in botanical
taxonomic schemes.) The earliest known protozoa lived in the
late Precambrian (see e.g. FORAMINIFERIDA).
The protozoa exhibit a great variety of forms, structures and
life styles, and are divided into seven phyla: APICOMPLEXA, ASCETOSPORA, CILIOPHORA, LABYRINTHOMORPHA, MICROSPORA, MYXOZOA and SARCOMASTIGOPHORA [JP (1980) 27 3758]. Many
protozoa are free-living organisms which occur in freshwater, brackish or marine habitats. Some protozoa occur e.g. in
soil, some are common in SEWAGE TREATMENT plants, and some
inhabit the gut in vertebrates or invertebrates (see e.g. RUMEN
and TERMITEMICROBE ASSOCIATIONS). Parasitic species include
e.g. members of the Apicomplexa, Ascetospora, Microspora and
Myxozoa; some protozoa are pathogenic in vertebrates (including man) or invertebrates (see e.g. BABESIA, BALANTIDIUM, EIMERIORINA, ENTAMOEBA, GIARDIA, HISTOMONAS, NAEGLERIA, NOSEMA,
PLASMODIUM, TOXOPLASMA, TRYPANOSOMA). PHYTOMONAS is parasitic in certain plants.
Protozoa range in size from ca. 1 m to several millimetres;
some have internal or external skeletons of e.g. calcareous,
siliceous and/or organic material. Many exhibit MOTILITY but
some (see e.g. PERITRICHIA) are sedentary. Probably most protozoa are aerobic organisms, but some can grow microaerobically
or anaerobically (see e.g. RUMEN and SAPROBITY SYSTEM). Feeding may occur saprotrophically and/or by pinocytosis and/or
it may occur holozoically (e.g. in many amoebae and ciliates),
these organisms being classified as CARNIVOROUS, HERBIVOROUS
or OMNIVOROUS. Some protozoa (see PHYTOMASTIGOPHOREA) can
carry out PHOTOSYNTHESIS.
Asexual reproduction may involve binary fission, multiple
fission and/or budding. Sexual processes occur in some species
(see e.g. AUTOGAMY and CONJUGATION). According to species,
protozoa may be haploid, diploid or polyploid; some (the
foraminifera) exhibit an ALTERNATION OF GENERATIONS.
Populations of viable protozoa may be preserved by FREEZING
(suitable e.g. for Plasmodium, Tetrahymena, Trypanosoma) or
by repeated subculturing. CYST-forming species (e.g. Didinium,
certain amoebae) may be encouraged to encyst (and thus survive
for protracted periods) e.g. by slow desiccation or by starvation.
protrichocyst Syn. EJECTOSOME.
Providencia
A genus of Gram-negative bacteria of the tribe
PROTEEAE. Cells: ca. 0.60.8 1.52.5 m. Swarming does
not occur. Species do not produce H2 S or lipase, do not
but those from previously infected cells can support phage replication. (See also SPHAEROPLAST; AUTOPLAST; L-FORM; PROTOPLAST
FUSION.)
(2) In an intact cell: the cytoplasmic membrane and all
structures internal to it.
protoplast fusion A technique for in vitro genetic transfer in
which a hybrid PROTOPLAST (and ultimately a hybrid cell) is
formed by fusing protoplasts derived from different strains,
species or genera. Protoplasts are initially prepared e.g. by
treating cells with wall-degrading enzymes (e.g. LYSOZYME for
some Gram-positive bacteria); populations of two types of
protoplast are then mixed. Treatment of the mixture with e.g.
POLYETHYLENE GLYCOL (PEG) increases the (low) spontaneous
rate of fusion. (cf. ELECTROFUSION.) The protoplasts are then
transferred to an appropriate (hypertonic) solid medium for cell
wall regeneration. The resulting cells can be screened for those
with genetic markers from both parents; e.g., if both parents
were auxotrophic (with different growth requirements) the cells
can be screened for prototrophs.
Hybrid bacterial protoplasts, containing a genome from each
parent, are called biparentals. The two genomes may undergo
recombination, or the diploids may be unstable, the two genomes
segregating when the cell divides. In e.g. Bacillus subtilis,
many of the progeny cells are unstable complementary diploids
(i.e., genes on both genomes are expressed and can exhibit
COMPLEMENTATION); however, some progeny cells are unstable
non-complementing diploids (Ncd cells) in which one of the two
parental genomes is expressed while the other is inactive until
segregated on cell division. (cf. CONJUGATION sense 1b (ii).)
(See also TRANSFORMATION.)
protoplast membrane Syn. CYTOPLASMIC MEMBRANE.
protoporphyrins See PORPHYRINS.
Protosporangium See PROTOSTELIOMYCETES.
Protostelia See EUMYCETOZOEA.
protostelids See PROTOSTELIOMYCETES.
Protosteliia See EUMYCETOZOEA.
Protosteliomycetes (protostelids) A class of primitive slime
moulds (division MYXOMYCOTA cf. EUMYCETOZOEA) in which
the vegetative phase consists of a small reticulate plasmodium or of simple amoebae which form filose and sometimes
also lobose pseudopodia; in some species the amoebae bear
one or more smooth flagella. Shuttle streaming (i.e., rhythmic
reversible flow of protoplasm) does not occur. An individual
amoeba, or a segment of a plasmodium, gives rise to a fruiting
body consisting of one to several spores borne on a slender
tubular stalk, the whole being bounded by a sheath. Ballistospores are formed e.g. by Protostelium nocturnum [Mycol.
(1984) 76 443447], P. expulsum [TBMS (1981) 76 303309],
and Schizoplasmodium cavostelioides [sporocarp ultrastructure
and development: Mycol. (1985) 77 848860]. [Ultrastructural study of trophozoite and cyst stages of P. pyriformis: JP
(1986) 33 405411.] Protostelids are found in various habitats, including bark, rotting wood, etc. Other genera include
e.g. Cavostelium, Ceratiomyxella, Endostelium [Mycol. (1984)
76 884891], Nematostelium and Protosporangium. (cf. CERATIOMYXA.)
Protostelium See PROTOSTELIOMYCETES.
Prototheca A genus of unicellular eukaryotic microorganisms
which are generally regarded as achlorophyllous strains of
CHLORELLA. The cells are hyaline and roughly spherical or ovoid
(ca. 1.313.4 1.316.0 m, depending on species, growth
conditions etc); when mature, a cell divides to form 220 or
more endospores which are released by rupture of the mother
623
provirus
liquefy gelatin at 22 C, and can metabolize mannose and one
or more sugar alcohols; colonies on DCA typically develop
yellow-orange centres due to the precipitation of Fe(OH)3 by
alkaline metabolic products. Nicotinic and pantothenic acids
are not required for growth. GC%: 3942. Type species:
P. alcalifaciens.
P. alcalifaciens (formerly included in Proteus inconstans).
Urease ve (weak or delayed Cve in a few strains); trehalose
ve; inositol. ve; adonitol Cve.
P. rettgeri (including most of the strains formerly regarded
as Proteus rettgeri ). Urease Cve; trehalose ve; inositol Cve;
adonitol Cve.
P. stuartii (incorporating strains formerly included in Proteus
inconstans and Proteus rettgeri ). Urease ve (weak or delayed
Cve in a few strains); trehalose Cve; inositol Cve; adonitol ve.
Providencia spp are rare in the normal human intestine,
and their natural habitat is unknown. Some strains can be
opportunist pathogens P. rettgeri and P. stuartii causing e.g.
nosocomial UTIs, P. alcalifaciens being more often associated
with diarrhoeal illnesses.
[Book ref. 22, pp. 494496.]
provirus Viral DNA which has become integrated into the chromosomal DNA of the host cell; in viruses of the RETROVIRIDAE
the DNA is a transcript of the RNA genome, while in some
DNA viruses the genome itself, or a portion of the genome, may
integrate (see e.g. DEPENDOVIRUS, HEPATITIS B VIRUS and MASTADENOVIRUS).
prozone (serol.) (1) In a titration involving antibodies and particulate antigens: absence of visible AGGLUTINATION in tubes containing the higher concentration(s) of antibody. A prozone may
be due e.g. to (i) relatively low titres of BLOCKING ANTIBODIES
(sense 1) which are diluted out in tubes containing agglutinating titres of normal homologous antibodies; (ii) gross ANTIBODY
EXCESS; or (iii) the presence in the antiserum of substances which
inhibit agglutination non-specifically.
(2) In a titration involving antibodies and soluble antigens:
the absence of visible precipitate in those tubes in which there
is an ANTIGEN EXCESS.
prozygosporangium See ZYGOSPORE.
PrP 2730 (PrP) See SCRAPIE.
PrPc , PrPsc See PRION.
PRRS Porcine reproductive and respiratory syndrome: see BLUEEARED PIG DISEASE.
pruinose (of surfaces) Powdery in appearance.
Prunus necrotic ringspot virus See ILARVIRUSES.
pruritis Itching.
Pruteen See SINGLE-CELL PROTEIN.
Prymnesiida See PHYTOMASTIGOPHOREA.
Prymnesiophyceae (Haptophyceae) A class of unicellular, uninucleate, commonly biflagellated algae (sometimes regarded as
protozoa see PHYTOMASTIGOPHOREA). Typically, the motile cell
has two smooth flagella of more or less equal length, together
with a HAPTONEMA; the golden-brown chloroplasts (usually two
per cell) contain chlorophylls a, c1 and c2 , and fucoxanthin.
Storage compounds include CHRYSOLAMINARIN. Many members
can ingest food phagocytically. Most prymnesiophytes bear
a covering of delicate, typically oval scales embedded in a
mucilaginous matrix external to the plasmalemma; these scales
are produced in the Golgi apparatus (or in vesicles probably
derived therefrom) before being passed to the cell exterior
(cf. CHRYSOPHYTES). The scales may be entirely organic (e.g.
in Chrysochromulina and Prymnesium) or may be calcified
(in certain stages of the COCCOLITHOPHORIDS). Some of the
Pseudomonas
pseudocapillitium In the aethalia or pseudoaethalia of certain
MYXOMYCETES: a system of threads (generally irregular in width)
and/or of membranous or perforated plate-like structures present
among the spores; it has been suggested that these structures
may be remnants of sporangial walls.
pseudocatalase A non-haemoprotein substance which catalyses
the breakdown of H2 O2 into water and O2 ; pseudocatalases
occur e.g. in various lactic acid bacteria, including strains of
Lactobacillus, Enterococcus faecalis, and in some species of
Veillonella. Unlike CATALASE, pseudocatalases are not inhibited
by low concentrations of azide or cyanide. A manganesecontaining protein pseudocatalase (a manganicatalase) has been
isolated from a strain of Lactobacillus plantarum [JBC (1983)
258 60156019].
Pseudocercosporella
See HYPHOMYCETES; see also EYESPOT
(sense 2).
pseudocilia See TETRASPORA.
pseudocoagulase In certain strains of Staphylococcus: any protease that mimics the effects of staphyloCOAGULASE by proteolytic activation of prothrombin, thus causing a false-positive
reaction in a COAGULASE TEST. Pseudocoagulase is believed to
be a metalloprotease(s) and can be inhibited by adding EDTA
to the plasma. [Book ref. 44, p. 530.]
pseudocolumella In the fruiting bodies of certain MYXOMYCETES:
a COLUMELLA-like, spherical or rod-shaped, calcareous structure
which occurs in the centre of the sporangium; it is not attached
to the peridium, but may be attached to capillitial threads.
pseudocowpox A mild, usually benign CATTLE DISEASE characterized by the formation of papular, scab-forming lesions on the
teats which may predispose to MASTITIS; the causal agent is a
PARAPOXVIRUS. (See also MILKERS NODULE; cf. COWPOX.)
pseudocyphella (lichenol.) A small pore (ca. 0.12.0 mm diam.)
in the (upper and/or lower) cortex of the thallus in various lichens
(e.g. species of Cetraria, Parmelia, Pseudocyphellaria). Pseudocyphellae have no definite margin (cf. CYPHELLA); they appear
to be formed by the disintegration of the pseudoparenchymatous
cortex, and are believed to facilitate gas exchange [Lichenol.
(1981) 13 110]. (cf. PORED EPICORTEX.)
Pseudocyphellaria A genus of foliose LICHENS (order PELTIGERALES) which closely resemble STICTA spp but differ in that the
tomentose underside is perforated with PSEUDOCYPHELLAE. The
upper surface may bear soredia which are yellow in P. crocata,
bluish-grey in P. intricata. Species occur on soil, trees, rocks,
etc.
pseudocyst (protozool.) See e.g. CHAGAS DISEASE and TOXOPLASMOSIS.
pseudoepithecium In some types of APOTHECIUM: a layer, at
the surface of the hymenium, which consists of the tips of
paraphyses immersed in an amorphous matrix. (cf. EPITHECIUM.)
pseudo-Fiji disease See FIJI DISEASE.
pseudogene In a eukaryotic chromosome: a DNA segment which
resembles a known functional gene but differs in carrying
deleterious mutations and in having no apparent function. Many
pseudogenes resemble cDNA copies of cellular mRNAs: they
have a short AT tract at the 30 end (corresponding to the 30 poly(A) of mRNA), lack introns, and are often flanked by direct
repeats; such pseudogenes are believed to have arisen by reverse
transcription of cellular mRNAs.
Pseudogenes have also been found in prokaryotes. For
example, in Mycobacterium leprae about 27% of the genome
is reported to consist of pseudogenes [Nature (2001) 409
10071011].
pseudoglanders Syn. EPIZOOTIC LYMPHANGITIS.
pseudohaemoptysis (pseudohemoptysis) The apparent expectoration of blood due to the coloration of sputum by red-pigmented
bacteria (e.g. Serratia sp).
Pseudohydnum See TREMELLALES.
pseudohyphae Syn. SPROUT MYCELIUM.
Pseudoklossia See EIMERIORINA.
pseudolumpy skin disease See LUMPY SKIN DISEASE.
pseudolysogeny A phenomenon in which an association between
a BACTERIOPHAGE and its host mimics LYSOGENY in that host
cell lysis is delayed or does not occur, but true lysogeny is not
established. A bacterial population exhibiting pseudolysogeny
can be freed of phage by prolonged incubation with neutralizing
anti-phage antiserum or by serial subculture from isolated
colonies. Different types of pseudolysogeny occur in different
phagebacterium systems. For example, when a population of
susceptible bacteria (e.g. Shigella dysenteriae) is exposed to a
virulent bacteriophage (e.g. T7) at a low multiplicity of infection,
a few cells become infected. On lysis, these cells may release
an enzyme which destroys the phage receptors on other cells
in the population; phage virions therefore fail to adsorb to
these cells which, as a result, become (temporarily) resistant
to infection (phenotypic resistance). These cells regain their
susceptibility to infection after subculture in the absence of
phage.
In other cases the phage genome may be carried, but not
expressed or replicated, within a cell in a susceptible population
of bacteria, and the genome is passed to only one of the daughter
cells at each cell division; a culture containing a proportion of
such carrier cells is known as a CARRIER CULTURE. After several
successive transits from cell to daughter cell, the phage genome
enters the lytic cycle and progeny phages are released by cell
lysis. These may infect other cells which may in turn become
carrier cells. This type of pseudolysogeny may occur e.g. when
most of the host cells are repressed for one or more functions
needed for phage replication.
In Azotobacter strain O certain phages can apparently establish a pseudolysogenic state accompanied by the phenotypic
conversion of the host cells (see BACTERIOPHAGE CONVERSION);
the cells lose their polysaccharide capsule, become flagellated
and motile, and acquire a yellow pigmented appearance [Virol.
(1980) 102 267277].
pseudomembranous colitis A severe, acute form of COLITIS.
There is a profuse, watery diarrhoea, cramps, fever, and the formation of pseudomembranous patches of inflammatory exudate
on the colonic mucosa (sometimes also in the small intestine).
It may follow chemotherapy (e.g. with some b-LACTAM ANTIBIOTICS, clindamycin) and is linked to CLOSTRIDIUM difficile; toxins
A and B kill gut epithelial cells e.g. by disrupting tight junction
proteins. Inadequate IgG response may promote disease/relapse.
[Review: BCG (2003) 17 475493.]
pseudomethylotroph An organism which oxidizes C1 compounds to CO2 and which assimilates C1 carbon only via the
Calvin cycle.
Pseudomicrothorax See HYPOSTOMATIA.
Pseudomonadaceae A family of Gram-negative, aerobic,
chemoorganotrophic or facultatively chemolithotrophic, typically motile (usually polarly flagellate), rod-shaped bacteria.
GC%: 5871. Genera: FRATEURIA, PSEUDOMONAS, XANTHOMONAS, ZOOGLOEA. [Book ref. 22, pp. 140219.]
Pseudomonadales A poorly defined, obsolete order of bacteria.
Pseudomonas A genus of Gram-negative, aerobic, chemoorganotrophic or facultatively chemolithoautotrophic bacteria of the
family PSEUDOMONADACEAE; species occur as free-living organisms in soil and aquatic habitats, and as pathogens in man,
625
Pseudomonas
groups IV. Group I included fluorescent species (e.g.
P. aeruginosa, P. aureofaciens, P. chlororaphis, P. putida,
P. syringae) and non-fluorescent species (e.g. P. alcaligenes,
P. pseudoalcaligenes, P. stutzeri ), all of which (apart from
some strains of P. pseudoalcaligenes) do not accumulate polyb-hydroxybutyrate (PHB). Species of groups II and III do
accumulate PHB; group II included pathogens (e.g. P. cepacia,
P. mallei, P. solanacearum), while group III consisted of nonpathogens (e.g. P. acidovorans, P. testosteroni ) and included
some autotrophs which can grow chemolithotrophically (e.g.
P. facilis, P. flava, P. paleronii and P. saccharophila). Group
IV consisted of P. diminuta and P. vesicularis, while group V
contained only P. maltophila; these three species require growth
factors, and the last two are unable to assimilate nitrate. For
group II see BURKHOLDERIA. For group V see P. maltophila,
below.
Many species have not been assigned to rRNA groups, and
their relationship to rRNA-grouped species is uncertain; such
species include e.g. P. agarici, P. amygdali, P. andropogonis,
P. aurantiaca, P. avenae, P. cattleyae, P. fragi, P. fulva,
P. lemoignei, P. marina (see DELEYA), P. nautica, P. spinosa
and P. woodii.
P. aeruginosa (formerly P. pyocyanea). Occurs in soil, river
water etc, and is an important opportunist pathogen in man and
other animals being isolated from infected burns, urinary tract
infections, etc. (See also BLUE PUS; EXOENZYME S; EXOTOXIN A.)
It can occasionally be pathogenic in (stressed) plants. Motile
strains usually have one polar flagellum per cell; rarely nonmotile. Polarly fimbriate. Colonies on nutrient agar are often
roundish, flat, dull and butyrous (R-type), but can be e.g. smooth
and umbonate (S-type). Mucoid (M-type) colonies are formed by
ALGINATE-producing strains isolated e.g. from CYSTIC FIBROSIS
patients; only some mucoid strains can produce alginate on
minimal agar. Most strains produce PYOCYANIN, and may also
produce e.g. PYOVERDIN, while a few strains can form a brown
pigment (pyomelanin) or a red pigment (pyorubin). (Pyomelanin
production is enhanced in mineral salts media containing 1% Ltyrosine; 1% DL-glutamate enhances pyorubin production.) All
strains are catalase Cve and oxidase Cve; many are urease Cve.
Optimum growth temperature: 37 C; all strains can grow at
42 C. GC%: ca. 67.
The production of virulence factors by P. aeruginosa may be
inhibited through inhibition of the organisms QUORUM SENSING
mechanisms by the macrolide antibiotic azithromycin [AAC
(2001) 45 19301933].
P. alcaligenes. A non-fluorescent species which cannot utilize
e.g. glucose, fructose, maltose or gluconate, but which can
use e.g. L-arginine, malate, and propionate. Monotrichously
flagellate. Growth can occur at 41 C; optimum temperature ca.
35 C. GC%: 6468.
P. andropogonis (D P. stizolobii ). A non-fluorescent, typically oxidase ve species pathogenic e.g. for sorghum. The
organisms form sheathed flagella at ca. 28 C but are nonflagellate when grown at 34 C.
P. carboxydohydrogena. See CARBOXYDOBACTERIA.
P. carboxydovorans. See CARBOXYDOBACTERIA.
P. cepacia. A former species (see BURKHOLDERIA) found e.g.
in soil, water. Oxidase Cve. Lophotrichously flagellate. Nonfluorescent pigments often formed. Opt. growth: 3035 C.
Pathogenic in man (see CYSTIC FIBROSIS) and a causal agent of
soft rot in onions.
P. cichorii. A fluorescent, PYOVERDIN-forming species pathogenic for chicory: Lophotrichously flagellate. Weakly oxidase
Cve. Optimum growth temperature: ca. 30 C. GC%: 59.
other animals, and plants see e.g. BLUE PUS, BROWN BLOTCH,
GINGER BLOTCH, OLIVE KNOT and TABTOXIN. [Mechanisms of
plant pathogenesis: CJM (1985) 31 403410.] (See also BUTTER and MEAT SPOILAGE.) The cells are straight or slightly
curved rods, 0.51.0 1.55.0 m. In most species the majority of strains are motile with one or several unsheathed polar
flagella per cell; however, sheathed flagella are formed e.g.
by P. andropogonis, and some species produce both polar
and lateral flagella particularly when grown on solid media.
[Biochemical and serological properties of flagella of some Pseudomonas spp: JGM (1985) 131 873883.] Polarly fimbriate
strains may exhibit TWITCHING MOTILITY. Cell walls and cytoplasmic membranes resemble those of other Gram-negative bacteria.
(See also PORIN, OUTER MEMBRANE and S LAYER.) Catalase Cve;
many strains are oxidase Cve. GC%: 5870. Type species:
P. aeruginosa.
Nutrition, metabolism, growth. Typically, the organisms are
nutritionally and metabolically highly versatile: most species
will grow on inorganic salts with an organic carbon source,
while some can grow chemolithoautotrophically; however, certain species (e.g. P. diminuta, P. vesicularis) require factors such
as biotin, cyanocobalamin and pantothenate. Metabolism is respiratory (oxidative); many species can carry out NITRATE RESPIRATION. The TCA CYCLE operates in all species investigated. In e.g.
P. aeruginosa, P. fluorescens and P. putida, glucose can be oxidized by EXTRACYTOPLASMIC OXIDATION to gluconate which may
then be metabolized via the ENTNERDOUDOROFF PATHWAY. Carbohydrates are metabolized anaerogenically. [Alternative pathways of carbohydrate metabolism in Pseudomonas: ARM (1984)
38 359387.] HYDROCARBONS can be metabolized by some
strains. Some metabolic activities are plasmid-dependent: e.g.,
the ability to degrade camphor, salicylate, toluate and xylene is
associated with plasmids CAM, SAL, TOL and XYL, respectively. Under nitrogen-limiting conditions some species accumulate POLY-b-HYDROXYBUTYRATE. Under iron-deficient conditions,
siderophores (some fluorescent) may be secreted (see NOCARDAMINE, PYOVERDIN). (See also PYOCYANIN.) Some species produce bacteriocins (see e.g. PYOCIN). In many species growth
occurs optimally at ca. 2830 C and is generally inhibited at
or below ca. pH 4.5.
Sensitivity to antimicrobial agents. In general, pseudomonads
are resistant to a range of common antimicrobial agents;
resistance may or may not be plasmid-mediated. P. aeruginosa
may be sensitive to e.g. certain AMINOGLYCOSIDE ANTIBIOTICS
(e.g. amikacin, gentamicin); it is resistant to many common
DISINFECTANTS (cf. DETTOL CHELATE) but is usually lysed rapidly
by EDTA.
Susceptibility to phages. Pseudomonas spp are susceptible to
a variety of phages: see e.g. BACTERIOPHAGE f6; BACTERIOPHAGE
fW-14; INOVIRUS; TECTIVIRIDAE. The transducing phages F116 and
G101 were used for mapping the chromosome of P. aeruginosa.
Lysogeny is very common in P. aeruginosa, but is uncommon
in other species.
Genetic aspects. Genetic studies have often been carried
out with P. aeruginosa strain PAO. [Chromosomal maps of
P. aeruginosa PAO and P. putida PPN compared: JGM (1985)
131 885896.] Gene transfer can occur by transduction and
conjugation; most conjugative plasmids transfer better on solid
media than in liquids [JGM (1983) 129 25452556]. Transformation in P. aeruginosa has been achieved with CaCl2 -treated
cells.
Taxonomy. A number of pseudomonads were classified
by rRNA oligonucleotide cataloguing (q.v.) into rRNA
626
pseudopodetium
pisi (peas); P. syringae pv. savastanoi (olive trees see OLIVE
P. syringae pv. syringae (lilac) (see also SYRINGOMYCIN);
P. syringae pv. tabaci (tobacco see TABTOXIN).
P. thermocarboxydovorans. See CARBOXYDOBACTERIA.
P. tolaasii. The causal agent of BROWN BLOTCH in mushrooms.
[Book ref. 22, pp. 140199; ecology, isolation, culture: Book
ref. 45, pp. 655741; the biology of Pseudomonas: Book
ref. 198.]
pseudomonic acid A Syn. MUPIROCIN.
pseudomurein A CELL WALL polymer present in some members
of the ARCHAEA (METHANOBACTERIALES); it consists of (1 ! 3)b-linked backbone chains containing N-acetyl-D-glucosamine
(and/or N-acetyl-D-galactosamine, according to species) and Nacetyl-L-talosaminuronic acid cross-linked by peptides which
contain only L-amino acids (lys, glu, ala or thr). (cf. PEPTIDOGLYCAN.) Pseudomurein is resistant to LYSOZYME and to
antibiotics such as penicillins and vancomycin. [Book ref. 157.
pp. 416423.]
pseudomycelium Syn. SPROUT MYCELIUM.
pseudonavicella See MONOCYSTIS.
pseudonigeran A water-insoluble, alkali-soluble (1 ! 3)-a-Dglucan present in the CELL WALL in certain fungi: e.g.
Aspergillus nidulans, Paracoccidioides brasiliensis (yeast form),
Schizophyllum commune. Pseudonigeran can act as a reserve
carbohydrate for cleistothecium formation in the teleomorph of
A. nidulans (Emericella nidulans). (cf. NIGERAN.)
Pseudonocardia A genus of bacteria (order ACTINOMYCETALES,
wall type IV) which occur e.g. in manure and soil. The organisms
form non-fragmenting substrate mycelium, and unbranched
aerial hyphae which give rise to chains of cylindrical spores.
Mycolic acids are not formed. GC%: ca. 79. Type species:
P. thermophila. [Book ref. 73, pp. 125126; ecology, isolation,
cultivation: Book ref. 46, pp. 21032117.]
pseudoparaphysis A type of sterile, typically branched and
anastomosing, usually septate filament (of unknown function)
which originates in the upper wall of a pseudothecial locule and
grows downwards between the asci, subsequently fusing with
the lower wall. (cf. PARAPHYSIS; see also HAMATHECIUM.)
pseudoparenchyma See PLECTENCHYMA.
pseudoperithecium See ASCOSTROMA.
Pseudoperonospora See PERONOSPORALES.
pseudopilins Certain components of the SECRETON which exhibit
a region of homology with the pilins of type IV fimbriae;
homology is limited to the 30 (hydrophobic) amino acids found
at the N-terminal of the protein, i.e. those residues which, in the
pilins, interact during fimbrial assembly.
Studies on those bacteria which encode both the secreton and
type IV fimbriae suggested that a functional relationship may
exist between the operation of the secreton and the mechanism of
fimbriation. Subsequently, when genes encoding the pullulanase
secreton of Klebsiella oxytoca were expressed in Escherichia
coli K-12, one of the pseudopilins, PulG, was found to assemble
into a pilus-like structure [EMBO (2000) 19 22212228].
pseudoplasmodium (1) A multicellular, commonly motile structure formed by the aggregation of amoeboid cells (prior to
fruiting) in CELLULAR SLIME MOULDS. (2) The ectoplasmic net
of members of the LABYRINTHULOMYCETES. (3) In the MYXOBACTERALES: a number of individual cells embedded in a slime
matrix.
pseudopodetium (lichenol.) A vertical, fruticose, branched or
unbranched, usually solid secondary thallus which develops by
growth from the primary thallus and is thus a purely thalline
(vegetative, somatic) structure (cf. PODETIUM); ascocarp initials
KNOT);
627
pseudopodium
develop on the pseudopodetia. Pseudopodetia occur e.g. in
species of PILOPHORUS and STEREOCAULON.
pseudopodium An extension of an amoeboid cell formed by
extrusion of the cytoplasm (bounded by the plasmalemma).
Pseudopodia are characteristically formed by protozoa of the
SARCODINA; according to species, pseudopodia may function in
locomotion and/or in feeding, and one or more may be formed
at a time by a given cell. Various types of pseudopodia are
formed by sarcodines. A lobopodium (lobose pseudopodium)
is blunt-ended and generally broad, and often has a clear
ectoplasmic area (the hyaline cap); lobopodia may be formed
eruptively, i.e., by a burst of cytoplasmic movement, or more
slowly by a steady cytoplasmic flow. A filopodium (filose
or filiform pseudopodium) is slender, filamentous, sometimes
tapered and sometimes branched, but lacks rigid axial elements
(cf. AXOPODIUM) although it may contain microtubules. Fine,
filamentous pseudopodia which branch and anastomose to form
a network are called reticulopodia or rhizopodia. In some
sarcodines more or less fine subpseudopodia may arise from a
broader pseudopodial lobe (see e.g. ACANTHAMOEBA).
In e.g. Amoeba proteus (see AMOEBA) the lobose pseudopodia
function in both feeding and locomotion. When a prey organism
comes into the vicinity of a pseudopodium, the pseudopodium
flows around it, initially forming a cup (food cup) containing the prey; the plasmalemma eventually closes around the
prey to form a FOOD VACUOLE. (cf. AXOPODIUM.) Locomotion in
A. proteus involves the extension of pseudopodia which apparently adhere to the substratum; cytoplasm then continues to flow
into one of the pseudopodia, which expands to accommodate it,
and further pseudopodia are extended, etc. This type of locomotion is often regarded as typical amoeboid movement, although
other forms of motility occur in other sarcodines. For example, in
Pelomyxa the cell moves along by steady cytoplasmic flow without the formation of obvious pseudopodia. (See also HELIOZOEA
and TAXOPODIDA.) Apart from functioning in active motility,
pseudopodia in some amoebae (e.g. Vannella spp) can apparently function as flotation devices; such amoebae can, under
certain conditions, produce distinct flotation forms characterized by fine, usually hyaline pseudopodia which radiate from the
central cell mass.
The mechanism of pseudopodial movement is not understood.
It appears to involve microfilaments of ACTIN which lie just
beneath and which interact with the plasmalemma.
pseudorabies Syn. AUJESZKYS DISEASE.
pseudoraphe See DIATOMS.
pseudorinderpest Syn. PESTE DES PETITS RUMINANTS.
pseudorubella Syn. EXANTHEM SUBITUM.
pseudoseptum See SEPTUM (b).
pseudospores See USTILAGINALES.
pseudostem See PHALLALES.
pseudotemperate bacteriophage A BACTERIOPHAGE which can
establish PSEUDOLYSOGENY.
pseudothecium See ASCOSTROMA.
Pseudotrebouxia A genus of sarcinoid unicellular green algae
(division CHLOROPHYTA) which occur as photobionts in many
LICHENS. The cells are more or less spherical (up to ca. 30 m
in diam.). Pseudotrebouxia spp closely resemble TREBOUXIA
spp except in that asexual reproduction occurs not only by
the formation of zoospores and aplanospores but also by
vegetative cell division, i.e., basically, the division of one
cell into two non-motile vegetative cells, etc the resulting
cells remaining in contact (at least initially) to form sarciniform
groupings. [Pseudotrebouxia species in lichens, and discussion
of vegetative cell division: Lichenol. (1981) 13 6586.]
PTS
PTS (phosphoenolpyruvate-dependent phosphotransferase system)
A TRANSPORT SYSTEM, found in both Gram-negative and Grampositive bacteria, in which the substrate (e.g. a hexose, disaccharide or hexitol) is phosphorylated in a reaction which is an
essential part of the transport process. The source of energy (and
of phosphate) is normally phosphoenolpyruvate (PEP); the formula of PEP is given in Appendix I(a). (Certain enzymes can
generate PEP from ATP or GTP.)
In members of the Enterobacteriaceae, sugars whose uptake
is PTS-dependent (PTS sugars) include glucose, fructose,
mannose, mannitol, sorbitol, glucosamine, N-acetylglucosamine
and N-acetylmannosamine. (cf. LACTOSE.) (Lactose is a PTS
sugar e.g. in Staphylococcus aureus.)
Because sugars are often metabolized via their phosphate derivatives e.g. glucose 6-phosphate in Appendix
I(a) phosphorylation during uptake is a positive aspect of PTS
transport. (Note, however, that a non-metabolizable substrate
may be phosphorylated and transported by a PTS e.g. the sugar
analogue methyl a-glucoside can be transported by the glucosePTS of Escherichia coli and of Clostridium pasteurianum.) (See
also STREPTOZOTOCIN.)
A PTS consists of both cytoplasmic (soluble) and membranebound protein components; the early nomenclature for PTS components (enzymes I, II and III) has been somewhat modified. In
the simplest case (mannitol uptake in E. coli: see diagram), PEP
feeds energy and phosphate into the PTS by sequential phosphorylation of two soluble energy-coupling proteins: enzyme
I (here designated I) and a histidine-containing protein, HPr
(here designated H). (Genes encoding I and H occur in the
same (pts) operon.) The phosphate and energy are transferred
from H to a sugar-specific permease (the so-called II complex) in the cytoplasmic membrane; the permease includes a
transmembrane component (IIC), involved in the binding and
translocation of substrate, and two phosphorylation sites (IIA,
IIB) phosphorylation and concomitant transport (uptake) of
mannitol apparently occurring only at the IIB site.
Uptake of glucose by PTS (see diagram) differs in that the
IIA component is soluble adding a further cytoplasmic step to
the chain of phosphorylation.
Phosphorylated forms of components I and H have high free
energies of hydrolysis (approximately that of PEP). The I and
H components are not substrate-specific, i.e. they are required
for the phosphorylation and transport of all PTS substrates; thus,
mutation causing loss of one or both of these components will
be pleiotropic, i.e. the mutant will be unable to transport any
PTS-dependent substrate. In contrast, inactivation of a given II
complex will affect the transport of only the relevant permeasespecific substrate(s).
[PTS (review): Mol. Microbiol. (1994) 13 755764.]
In enterobacteria, some complex II components apparently
contain oxidizable sulphhydryl groups, and it seems that only
reduced forms are active [Biochem. (1985) 24 4751]; this may
indicate an energy-dependent regulation of the PTS, and may
account for the observed pmf-related regulation of PTS activity.
In some II complexes the components are grouped in other
ways. For example, the fructose permease of enteric bacteria
consists of a membrane-bound protein, containing IIC and IIB,
and a separate protein containing the functions of both IIA and
HPr. In Rhodobacter capsulatus, the fructose permease includes
a single protein which carries out the functions of IIA, HPr and
enzyme I.
629
glucose
IIC
IIA
CM
IIC
IIB
IIB
mannitol
1-phosphate
H
H
IIA
glucose
6-phosphate
P
P
PEP
PTS (phosphoenolpyruvate-dependent phosphotransferase system). Transport of mannitol and glucose across the cytoplasmic membrane
(CM) by the PTS in Escherichia coli (simplified, diagrammatic); transport is from the periplasm (above) to the cytoplasm (below). Note that
mannitol and glucose are taken up by different membrane-associated systems (permeases).
P
The source of energy for transport is phosphoenolpyruvate (PEP). Energy is fed into the system by the sequential transfer of phosphate
from PEP to enzyme I (shown here as I) and then to the HPr protein (shown here as H). In mannitol transport, phosphate is transferred from H
direct to a membrane-bound permease (enzyme II complex, here designated II). The permease for mannitol consists of three domains: IIA, IIB
and IIC. IIC is a hydrophobic, transmembrane domain which binds the specific substrate and appears to contain, or contribute to, a channel
through which the substrate is translocated. The IIA and IIB domains each contain a phosphorylation site, but phosphorylation of the substrate
seems directly to involve only the IIB domain.
In the glucose permease, IIA is a separate (cytoplasmic, soluble) protein; however, the sequence of phosphorylation is the same as that in
the mannitol permease, i.e. IIA ! IIB ! substrate.
In all cases, phosphorylation of the substrate is an integral part of the transport mechanism.
Reproduced from Bacteria, 5th edition, Figure 5.12, page 91, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
putrefaction
pulpwood spoilage See PAPER SPOILAGE.
pulpy kidney An acute toxaemic disease of ruminants (especially
lambs) caused by growth and toxigenesis by Clostridium perfringens type D in the intestines. Symptoms: diarrhoea, convulsions,
paralysis, sudden death.
pulque A white, viscous, acidic, alcoholic Mexican beverage
made by fermenting the juices of Agave spp. The alcohol
is produced by Saccharomyces cerevisiae (S. carbajali ) and
Zymomonas mobilis. Acidity and viscosity are contributed,
respectively, primarily by Lactobacillus plantarum and dextranproducing strains of Leuconostoc. Pulque is rich in B vitamins.
Tequila is made by the distillation of pulque. (See also WINEMAKING; SPIRITS.)
pulsechase technique A technique in which e.g. living cells
are exposed to a pulse of labelled substrate for a fixed period
of time followed immediately by a high concentration of the
unlabelled substrate (the chase phase); the chase effectively
stops further uptake/use of the labelled substrate, thus defining
the duration of the pulse. The technique has been used e.g. to
follow the intracellular movement of a secreted protein from the
time of its synthesis to the time of secretion; for this experiment,
the period of the pulse is increased in a stepwise manner.
pulsed electric field (PEF) A technique involving electric fields
of typically >20 kV/cm applied in pulses of up to several s
(microseconds) for the inactivation of susceptible microorganisms in a liquid medium; exposure to PEF treatment appears
to bring about irreversible structural damage to the cells. In
one experiment, the use of 2500 pulses of a 30 kV/cm field
at 50 C reduced the level of viable cells of Mycobacterium
paratuberculosis in milk by ca. 5.9 log10 cfu/ml [AEM (2001)
67 28332836].
This technique may have applications e.g. in the food industry.
pulsed-field gel electrophoresis See PFGE.
pulverulent Powdery.
pulvinate Cushion-like; forming a swelling.
pulvomycin See POLYENE ANTIBIOTICS (b).
punctate Having surface dot(s), pore(s) etc.
punctiform Dot-like.
Punta Toro virus See PHLEBOVIRUS.
PUO Pyrexia (fever) of unknown origin.
pure culture See CULTURE.
purified protein derivative See TUBERCULIN.
purine nucleotide biosynthesis See NUCLEOTIDE and Appendix V(a).
purity plate A plate inoculated from a given culture and subsequently incubated to determine whether the culture was pure or
contaminated the presence of two or more types of colony on
the purity plate indicating a contaminated culture.
puromycin (6-dimethyl-30 -deoxy-30 -p-methoxyphenylalanylamino
adenosine) A NUCLEOSIDE ANTIBIOTIC obtained from Streptomyces alboniger or synthesized chemically; it is active against
prokaryotes and eukaryotes. It acts primarily as an inhibitor of
PROTEIN SYNTHESIS, acting as an analogue of the aminoacyl-adenyl
portion of an aminoacyl-tRNA. When a peptidyl-tRNA occupies
a ribosomal P site, puromycin can enter the A site and a peptide
bond can be formed between the amino group of puromycin and
the C-terminus of the peptide. However, puromycin does not have
a hydrolysable ester bond like that linking the aminoacyl group to
a tRNA, and puromycin binds only weakly to the ribosome; thus,
nascent polypeptide chains (in which the C-terminus is blocked
by puromycin) are released.
purple bacteria (1) Bacteria of the RHODOSPIRILLINEAE. (2) A
category (D PROTEOBACTERIA q.v.) within the domain BACTERIA originally distinguished on the basis of 16S rRNA sequence
analysis [SAAM (1985) 6 143151]. Organisms in this category are believed to have evolved from photosynthetic bacteria
similar to members of the Rhodospirillineae; they are divided
into the alpha, beta, gamma, delta and epsilon subdivisions.
purple laver See LAVER.
purple membrane In some strains of Halobacterium salinarium:
functionally and structurally differentiated, purple-pigmented
regions of the cytoplasmic membrane which develop under
microaerobic or anaerobic conditions in the light; purple
membrane may occupy up to 50% of the total membrane
area the remaining cytoplasmic membrane (which contains red
carotenoid pigments) often being called the red membrane. The
purple membrane utilizes light energy to effect transmembrane
translocation of protons, thus generating or augmenting a proton
motive force (pmf) (see CHEMIOSMOSIS); cells can therefore grow
as phototrophs under anaerobic conditions (see HALOBACTERIUM).
The protein component of the purple membrane consists
almost entirely of BACTERIORHODOPSIN (q.v.) but includes another
retinal-containing purple pigment, HALORHODOPSIN, and (in
at least some cases) SLOW-CYCLING RHODOPSIN. (Strains of
H. salinarium which cannot synthesize retinal may form an
apoprotein-containing white membrane.)
The lipids of the purple membrane are similar to those in
the remainder of the cytoplasmic membrane, but they include
a glycosulpholipid which is apparently unique to the purple
membrane.
While photocycling in bacteriorhodopsin causes an outward
efflux of protons, photocycling in halorhodopsin appears to cause
an inward pumping of chloride ions (rather than an outward
pumping of sodium ions as was previously thought).
The combined activities of light-energized bacteriorhodopsin
and halorhodopsin may account for the various ion fluxes
across the membrane and for the complex pattern of changes
in transmembrane pH differential.
When whole cells are illuminated, the steady-state or resting
membrane potential (typically ca. 100110 mV) is increased by
ca. 1040 mV, and the resting transmembrane pH differential
(ca. 2 units at pH 5, ca. 0 units at pH 8) changes by
01 unit; the increased membrane potential serves to energize
e.g. photophosphorylation (phosphorylation of ADP), uptake of
potassium ions and efflux of sodium ions.
purple non-sulphur bacteria See RHODOSPIRILLACEAE.
purple sulphur bacteria See CHROMATIACEAE.
purpura (med.) A condition characterized by reddish or purple
patches due to haemorrhage into skin or mucous membrane and
underlying tissues. A pin-point-sized haemorrhage is called a
petechia, a larger one is known as an ecchymosis.
purse (mycol.) See CYATHUS.
purulent Containing, consisting of, or forming PUS.
pus A thick, usually yellowish, fluid product of inflammation
formed at the site of an infection. Pus contains proteins,
leucocytes, cell fragments, and e.g. living and/or dead bacteria.
(cf. BLUE PUS.)
pustulan A (1 ! 6)-b-D-glucan produced by Lasallia (Umbilicaria) pustulata.
pustule A small, raised, PUS-filled skin lesion. (cf. VESICLE.)
pusule In many DINOFLAGELLATES: an intracellular vesicular
structure which opens to the exterior via a canal and a pore;
it is believed to function in osmoregulation but is apparently
non-contractile (cf. CONTRACTILE VACUOLE).
putidaredoxin See FERREDOXINS.
putrefaction The microbial degradation of proteinaceous materials with the formation of evil-smelling products such as amines
631
putrescine
cysteine-HCl, NaCl, resazurin, and glucose (added after autoclaving), and may be used as a broth (PYGB) or as an agar
medium (PYGA). [Recipe: Book ref. 53, p. 1428.]
Py-GLC PYROLYSIS GASLIQUID CHROMATOGRAPHY.
pyknosis (pycnosis) (histopathol.) The shrinkage of a cells
nucleus, resulting in the formation of a smaller, densely staining
body. (cf. KARYOLYSIS; KARYORRHEXIS.)
pyo- Prefix meaning pus.
pyocin (pyocine; aeruginocin) Any BACTERIOCIN produced by
Pseudomonas aeruginosa; pyocins are bactericidal log-phase
target cells apparently being the most sensitive. R-type pyocins
(MWt ca. 107 ) resemble phage tails and are relatively insensitive
to proteases; S-type pyocins (MWt ca. 105 ) are amorphous and
are sensitive to proteases.
Pyocin typing: see BACTERIOCIN TYPING.
pyocyanin (pyocyanine) A blue-green, water-soluble and nonfluorescent phenazine pigment synthesized by Pseudomonas
aeruginosa from chorismate (an intermediate in the biosynthesis
of aromatic amino acids: see Appendix IV(f)); it becomes
red-purple when acidified. Pyocyanin has oxygen-dependent
antimicrobial activity which appears to involve the (enzymeindependent) oxidation of NADH with production of SUPEROXIDE
and H2 O2 [JB (1980) 141 156163]; it also inhibits the beating
of human respiratory cilia in vitro [JCI (1987) 79 221229].
(cf. CYANOMYCIN; see also IRON.)
pyoderma Any purulent skin disease e.g. IMPETIGO.
pyofluorescein Syn. PYOVERDIN.
pyogenic Able to cause formation of pus.
pyomelanin See PSEUDOMONAS (P. aeruginosa).
pyorubin See PSEUDOMONAS (P. aeruginosa).
pyoverdin (pyoverdine; pyofluorescein; fluorescein) Any of a
range of yellowish, fluorescent, water-soluble pigments produced
by certain species of Pseudomonas under iron-deficient conditions; the pyoverdins act as SIDEROPHORES.
A model for the iron-regulated induction of pyoverdin in
P. aeruginosa proposes that, under iron-deficient conditions,
the (regulatory) Fur protein dissociates from a transcriptional
control site upstream of the pvdS gene, allowing synthesis of
PvdS; PvdS is a sigma factor which promotes transcription of
genes involved in the synthesis of pyoverdin [JB (1996) 178
22992313].
The pyoverdin of P. fluorescens contains a quinoline chromophore linked to a cyclic peptide; this compound represses
synthesis of another siderophore, quinolobactin [AEM (2000)
66 487492].
[Functional analysis of PvdS: JB (2000) 182 14811491.]
PYR A substrate (N,N-dimethylaminocinnamaldehyde) which is
apparently hydrolysed by all strains of Streptococcus pyogenes
but by no other streptococci. In an identification test for
S. pyogenes, the organisms are grown aerobically on agar plates
overnight at 35 C; when PYR is added to the surface growth,
colonies of S. pyogenes become red, while those of other
streptococci become yellow or do not change colour.
PYR is also hydrolysed by strains of ENTEROCOCCUS.
Pyr(64)Pyo See ULTRAVIOLET RADIATION.
pyracarbolid (2H-3,4-dihydro-6-methylpyran-5-carboxanilide)
An agricultural systemic ANTIFUNGAL AGENT which is active e.g.
against various rusts, smuts, and Rhizoctonia spp.
Pyramimonas See MICROMONADOPHYCEAE.
pyrazinamide 1,4-Diazine carboxamide: a drug active against
Mycobacterium tuberculosis in vivo (including cells within
phagosomes) and (at e.g. pH 5.6) in vitro. M. bovis is not
susceptible.
Pyrrhophyta
Pyrazinamide is a prodrug which is converted, in vivo,
to the active compound pyrazinoic acid; conversion involves
the enzyme pyrazinamidase, which is encoded by gene pncA
in Mycobacterium tuberculosis. Most pyrazinamide-resistant
clinical isolates of M. tuberculosis have been found to have
mutations in the pncA gene.
Expression of M. smegmatis pyrazinamidase in mutant
(pyrazinamide-resistant) M. tuberculosis confers hypersensitivity to pyrazinamide and related amides [JB (2000) 182
54795485].
pyrazinoic acid See PYRAZINAMIDE.
pyrazophos An antifungal ORGANOPHOSPHORUS COMPOUND which
is active against various powdery mildews. It is readily absorbed
by leaves and shoots, and is translocated within the plant; it is
poorly absorbed by roots.
pyrBI, pyrE genes See OPERON.
pyrenoid A dense proteinaceous body which occurs within a
CHLOROPLAST; in some cases a pyrenoid may be stalked
protruding from the chloroplast but always contained by the
chloroplast envelope. The pyrenoid appears to be the site of
synthesis of storage polysaccharide; the enzyme RuBisCO has
been isolated as the main protein component of the pyrenoids in
some species.
Pyrenomycetes A class of ascomycetes characterized by the formation of unitunicate asci in a perithecium or a cleistothecium.
The class is not recognized in most modern taxonomic schemes.
Pyrenophora See DOTHIDEALES.
Pyrenula See PYRENULALES.
Pyrenulales An order of saprotrophic and lichenized fungi of
the ASCOMYCOTINA. Ascocarp: ascolocular and perithecioid (see
ASCOCARP). Asci: bitunicate. Ascospores: multiseptate. Genera:
e.g. Acrocordia, Pyrenula.
Pyricularia A genus of fungi of the HYPHOMYCETES; teleomorph:
Magnaporthe. P. oryzae, the causal agent of rice BLAST DISEASE,
forms a septate mycelium and gives rise to typically pyriform,
commonly biseptate conidia.
pyricularin Syn. PIRICULARIN.
pyridine haemochrome See CYTOCHROMES.
pyridine nucleotide coenzymes NAD (q.v.) and NADP.
pyridine nucleotide salvage cycle See NAD.
pyridoxal phosphate See PYRIDOXINE.
pyridoxamine See PYRIDOXINE.
pyridoxine (pyridoxin; vitamin B6 ; pyridoxol) A water-soluble
and photolabile VITAMIN: 2-methyl-3-hydroxy-4,5-di-(hydroxymethyl)pyrimidine; related compounds such as pyridoxal and
pyridoxamine (bearing, respectively, CHO and CH2 NH2
at the 4-position) may also be referred to as vitamin B6 .
The coenzyme form of the vitamin is pyridoxal 5-phosphate
(codecarboxylase); pyridoxamine 5-phosphate is involved
in some reactions. The coenzyme is important in amino
acid metabolism e.g., in reactions involving transamination,
decarboxylation, racemization (interconversion of D-and L-amino
acids), serineglycine interconversion, etc.
Certain microorganisms (e.g. Clostridium spp, Lactobacillus spp, some yeasts, Crithidia fasciculata, Tetrahymena spp)
require an exogenous supply of pyridoxine; the various derivatives are not necessarily equally effective in this respect.
pyridoxol Syn. PYRIDOXINE.
pyriform Pear-shaped.
pyrimethamine (2,4-diamino-5-(p-chlorophenyl)-6-ethylpyrimidine) A FOLIC ACID ANTAGONIST used usually in combination
with e.g. a sulphonamide in the treatment of MALARIA and
of toxoplasmosis and other coccidioses; it is active against the
trophozoite, but resistance tends to develop readily.
pyrrolo-(1,4)-benzodiazepine antibiotics
tube which penetrates the host plant giving rise to both intercellular and intracellular mycelium; haustoria are not formed.
Later, spherical or ovoid, non-deciduous sporangia develop,
in terminal or intercalary positions, on undifferentiated sporangiophores. A sporangium germinates by extruding a thin
tube which terminates in a thin-walled, bubble-like vesicle; the
multinucleate contents of the sporangium flow into the vesicle
where they differentiate into zoospores.
In sexual reproduction, a spherical oogonium and a smaller,
club-shaped or elongated antheridium develop on the hyphae in a
terminal or intercalary position. (Most species of Pythium appear
to be homothallic, but at least one species, P. sylvaticum, is heterothallic.) Meiosis is generally thought to occur in the gametangia. A fertilization tube develops between antheridium and oogonium, and a male nucleus passes into the oogonium where fertilization occurs. The resulting thick-walled oospore germinates
to form a germ tube which may terminate in a zoosporangium.
Pythium red rot See ALGAL DISEASES.
Pythonella See EIMERIORINA.
pyuria The presence of pus in the urine. Sterile pyuria (D
abacterial pyuria) is a condition in which pus is repeatedly
found in samples of urine from which no bacteria can be cultured
by routine methods; common causes are probably chlamydiae or
mycoplasmas.
pYV plasmid See VIRULON.
634
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
Q
Q (1) See TEMPERATURE COEFFICIENT. (2) QUEUOSINE. (3) Glutamine (see AMINO ACIDS).
Q-band (in ESR) See ELECTRON SPIN RESONANCE.
Q bases Bases formed by the modification of guanine in tRNA;
they contain a pentenyl ring attached (via NH) to the methyl
group of N-methylguanine. An example is queuine, the Q base
of QUEUOSINE. (See also Y BASES.)
Q-cycle (protonmotive Q-cycle) A hypothetical pathway originally proposed (as part of the classical respiratory LOOP MODEL)
to account e.g. for proton extrusion at Complex III of the mitochondrial ELECTRON TRANSPORT CHAIN; this pathway requires the
presence of oxidized and reduced forms of ubiquinone (UQ and
UQH2 , respectively) and the free radical, semiquinone (UQH).
In one form of the Q-cycle, an electron which enters the matrix
side of Complex III is taken up, together with one proton from
the matrix side, by UQH forming UQH2 . On passing to the
cytoplasmic side, UQH2 undergoes oxidation to UQH one proton being extruded, and one electron passing back to the matrix
side via b-type cytochromes; this electron, together with a proton from the matrix side, reduces UQ, thus regenerating UQH at
the matrix side. At the cytoplasmic side, the UQH formed from
UQH2 undergoes oxidation to regenerate UQ, one proton being
extruded, and one electron passing to cyt c1 .
[Thermodynamic and kinetic considerations of Q-cycle mechanisms: JBB (1985) 17 5164.]
Q enzyme A BRANCHING ENZYME which can convert amylose
into an amylopectin-type polysaccharide; it cannot introduce
branches into amylopectin. It occurs in certain algae and in
higher plants.
Q fever In man, an acute disease caused by Coxiella burnetii
(see COXIELLA). Infection may occur e.g. by the inhalation of
contaminated dust or the ingestion of contaminated milk. After
an incubation period of 23 weeks there is a sudden onset with
headache, malaise, fever, muscular pain, and (often) respiratory
symptoms (pneumonitis); there is no rash. Complications (e.g.
endocarditis) may occur but the disease is rarely fatal. Diagnosis
may include e.g. serological tests and/or attempts to culture
C. burnetii from blood or sputum samples. Tetracyclines and
chloramphenicol have been used therapeutically. Reservoirs of
infection occur e.g. in sheep and cattle and in argosid and ixodid
ticks. [Minireview: JMM (1996) 44 7778.]
[Goat-associated Q fever in Newfoundland: EID (2001) 7
413419.]
QAC See QUATERNARY AMMONIUM COMPOUNDS.
Qalyub group See NAIROVIRUS.
Qiagen plasmid kit Any of several commercial kits (marketed
by Qiagen GmbH, Hilden, Germany) used for isolating plasmids
from bacteria (e.g. Escherichia coli ); up to 20 g of plasmid
DNA can be isolated with the mini kit, and up to 10 mg can
be isolated with larger kits.
For E. coli (and other Gram-negative bacteria) the outer
membrane is initially disrupted by a TrisEDTA buffer. Then,
controlled lysis of the cytoplasmic membrane with SDS (sodium
dodecyl sulphate) permits release of plasmids and soluble
proteins etc. (but not chromosomal DNA); contaminating RNA
is digested with RNase A. SDS and proteins (but not plasmids)
are precipitated in buffer, and a cleared lysate (containing the
plasmids) is obtained by centrifugation. The spun lysate is
passed through Qiagen anion-exchange resin; the resin is washed
quats
Quevedo disease See POD ROT.
quinacrine A weakly basic, yellow fluorescent ACRIDINE dye
(chromophore: 2-methoxy-6-chloro-9-aminoacridine) which has
been used in the chemotherapy of e.g. malaria and giardiasis,
and which is used as a chromosome stain.
quinapyramine An anti-trypanosomal agent used e.g. for the
treatment of dourine.
quinghaosu See QINGHAOSU.
quinic acid See CHLOROGENIC ACID.
quinidine See QUININE.
quinine An alkaloid obtained from the bark of the Cinchona
tree; the sulphate and hydrochloride are ANTIMALARIAL AGENTS
effective against the intraerythrocytic stage (blood schizont) of
the parasite (Plasmodium).
The diastereoisomer of quinine, quinidine, is used in place of
quinine e.g. in the USA; compared to quinine it is less proteinbound but more cardiotoxic.
Quinine appears to interfere with the parasites detoxification
of ferriprotoporphyrin IX (FP). FP, formed when the parasite
digests haemoglobin, is able to lyse the parasite unless it is
detoxified by polymerization to insoluble granules of pigment
(see HAEMOZOIN); such polymerization seems to involve a
haem polymerase [Nature (1992) 355 108109], and the
quinoline-type drugs (including e.g. quinine) possibly inhibit
this enzymic activity. In a photoaffinity labelling experiment,
quinine competitively inhibited the binding of a chloroquine
analogue to specific proteins (perhaps haem polymerase?)
within parasitized erythrocytes suggesting the presence of
targets common to the quinoline-type antimalarial agents [JBC
(1994) 269 69556961].
8-quinolinol Syn. 8-HYDROXYQUINOLINE.
quinolobactin A SIDEROPHORE, from Pseudomonas fluorescens,
whose synthesis is repressible by pyoverdin [AEM (2000) 66
487492].
quinolone antibiotics A group of synthetic ANTIBIOTICS whose
targets are GYRASE [gyrase-targeted antibiotics: TIM (1997) 5
102109] and topoisomerase IV; each antibiotic contains a
substituted 4-quinolone ring.
The original antibiotics in this group cinoxacin, NALIDIXIC
ACID, OXOLINIC ACID and pipemidic acid are active mainly
against Gram-negative bacteria (but not against Pseudomonas
aeruginosa); being rapidly excreted in urine, they have been
used for treating UTIs caused by members of the Enterobacteriaceae. However, these drugs are not well absorbed when given
orally and/or are readily inactivated in the body; they have a
limited antibacterial spectrum, and resistance develops readily.
Antibiotics subsequently added to the group were fluorinated,
piperazinyl-substituted derivatives (so-called fluoroquinolones);
they include ciprofloxacin, enoxacin, norfloxacin, ofloxacin and
pefloxacin. Compared to the earlier quinolones, these drugs have
a wider spectrum of activity (being active against e.g. Pseudomonas aeruginosa and certain Gram-positive cocci, including MRSA), are effective at much lower in vivo concentrations
and are more stable in the body; moreover, resistance to these
drugs develops less readily. [Comparison of activities of various
quinolones: JAC (1985) 16 475484, 485490. Laboratory and
clinical evaluation of pefloxacin: JAC (1986) 17 (supplement B)
1118.]
The fluoroquinolone danofloxacin has been used e.g. against
Mycoplasma bovis in the treatment of CALF PNEUMONIA; little
resistance to danofloxacin has developed in M. bovis, although
significant levels of resistance have developed against other antiM. bovis antibiotics, including oxytetracycline, spectinomycin
and the macrolide tilmicosin [VR (2000) 146 745747].
disrupting the cytoplasmic membrane and (at high concentrations) by denaturing proteins. A QAC may be regarded as an
ammonium halide with four substituents: a long-chain alkyl
group (C8 to C18 for high antimicrobial activity) and short-chain
alkyl and/or benzyl or heterocyclic groups. QACs are bacteriostatic at low concentrations, bactericidal at high concentrations.
They are typically more active against Gram-positive than Gramnegative bacteria, are reported to be fungistatic, trypanocidal,
and active against certain viruses, but have little or no activity
against Mycobacterium tuberculosis, Pseudomonas aeruginosa
and bacterial endospores. They have a DILUTION COEFFICIENT of
1, and are inhibited e.g. by low pH, organic matter (serum, faeces etc), anionic detergents, soaps, phospholipids, and certain
cations (e.g. Ca2+ , Mg2+ ) which may compete for sites on the
(negatively charged) cell surface. Various substances, (e.g. agar,
glass) strongly adsorb QACs.
QACs are used e.g. for pre-operative skin cleansing and
surgical dressings, and for the disinfection of equipment used
in the food and dairy industries. They include e.g. benzalkonium chloride (= Zephiran, a mixture of alkyldimethylbenzylammonium chlorides) used e.g. as a preservative in
ophthalmic solutions; benzethonium chloride (a substituted benzalkonium chloride); Cetrimide (= Cetavlon, a mixture of
hexadecyl- (cetyl-), tetradecyl- and dodecyl-trimethylammonium
bromides); cetylpyridinium chloride (1-hexadecylpyridinium
chloride); CTAB (cetyltrimethylammonium bromide); Domiphen
bromide (dodecyldimethyl-2-phenoxyethylammonium bromide).
quats QUATERNARY AMMONIUM COMPOUNDS.
Quayle cycle Syn. RMP PATHWAY.
Queensland tick typhus In man, a tick-borne disease caused by
Rickettsia australis.
Quellkorper
Within the closed ascocarps of certain fungi: a
gelatinous mass of cells believed to be involved in the rupture
of the (mature) ascocarp wall.
quellung phenomenon A phenomenon originally described by
Neufeld for Streptococcus pneumoniae in which the bacterial
CAPSULE becomes more easily observable (appears darker) in
the presence of antiserum specific for the capsular material.
Antibodies mark the outer limit of the capsule by combining with
its outermost layer. Since in the absence of antibodies the capsule
may be invisible by microscopy, antibodies were originally
thought to cause the capsule to swell (Quellung = swelling);
in fact, little actual swelling appears to occur.
quench-freezing The process of rapidly FREEZING a specimen by
plunging it into a suitable CRYOGEN.
Querbalken Lysozyme-sensitive crossbands in the prosthecae of
species of Asticcacaulis and Caulobacter.
quercetin A mutagenic flavonol glycoside pigment widely distributed in plants; it binds non-covalently to and inhibits (F0 F1 )type PROTON ATPASES.
queuine See QUEUOSINE.
queuosine (Q) A hypermodified guanosine derivative (7-[4,5cis-dihydroxy-1-cyclopentene-3-aminomethyl]-7-deazaguanosine) present in the wobble position (see WOBBLE HYPOTHESIS)
of tRNAs for aspartic acid, asparagine, histidine and tyrosine in
most prokaryotic and eukaryotic organisms investigated (but not
in Saccharomyces cerevisiae). The Q BASE queuine pairs with
either C or U. Modification of G to Q in the wobble position of
a tRNA anticodon can influence codon selection by the tRNA
in vivo [EMBO (1985) 4 823827]. In eukaryotes, the tRNA
Q content is variable and correlates with certain developmental changes [e.g. in Dictyostelium discoideum: JGM (1984) 130
135144].
636
quinones
H
C
CH2
CH2
N
HO CH
CH2
CH3
NHCHCH2CH2CH2N(C2H5)2
CH3O
N
Cl
Quinine
Chloroquine
H
HO
HOCCH2CH2N(C4H9)2
HC
Cl
N
H
N
CF3
CF3
CF3
Mefloquine
Cl
Halofantrine
CH3
HNCH(CH2)3NH2
N
CH3O
Primaquine
QUININE and some other antimalarial drugs (see MALARIA for further details of these and other antimalarials).
Reproduced from Antimicrobial Drug Action, Figure 7.3, page 123, R.A.D. Williams, P.A. Lambert & P. Singleton (1996) copyright Bios
Scientific Publishers, UK (ISBN 1-872748-81-3) with permission from the publisher.
The activities of some of the newer fluoroquinolones (including gatifloxacin, grepafloxacin, levofloxacin, moxifloxacin and
trovafloxacin) have been ascertained against ciprofloxacinresistant Streptococcus pneumoniae; these newer drugs were
found to have improved activities compared with that of
ciprofloxacin [AAC (2001) 45 16541659].
Various drugs (including gatifloxacin, gemifloxacin, grepafloxacin, levofloxacin and moxifloxacin) are discussed in the
Report of the 7th International Symposium on New Quinolones
(Edinburgh, June 1012th, 2001) [JAC (2001) 47 (supplement
S1)].
(See also CcdB in F PLASMID.)
quinomycins See QUINOXALINE ANTIBIOTICS.
quinone antifungal agents A group of agricultural ANTIFUNGAL
AGENTS which includes e.g. BENQUINOX, CHLORANIL, DICHLONE
and DITHIANON.
quinones Aromatic dioxo (diketo) compounds which are typically coloured (usually yellow, orange or red) and are e.g.
constituents of many natural pigments. Quinones are classified
as benzoquinones, naphthoquinones etc according to the nature
of the aromatic ring system. Microorganisms contain a range of
637
quinoprotein
quinoprotein A class of ENZYME in which the prosthetic
group is pyrrolo-quinoline quinone (PQQ): 2,7,9-tricarboxy-1H pyrrolo(2,3f )-quinoline-4,5-dione. Quinoproteins include e.g.
methanol dehydrogenase (in which PQQ is called methoxatin),
and glucose dehydrogenase (EC 1.1.99.17). [PQQ and quinoproteins in microbial oxidations: FEMS Reviews (1986) 32
165178.] (See also EXTRACYTOPLASMIC OXIDATION and METHYLOTROPHY.)
quinovosamine 2-Amino-2,6-dideoxyglucose: a TRIFOLIIN Abinding component of LPS in strains of Rhizobium leguminosarum biotype trifolii.
quinoxaline antibiotics Bifunctional INTERCALATING AGENTS
(f ca. 48 ), each having two quinoxaline 2-carboxylic acid chromophores linked by a cyclic octapeptide dilactone containing Dand L-amino acids; the peptide has a central cross-bridge (thioacetal in the quinomycins, disulphide in the triostins). The two
parallel chromophores project from the (relatively rigid) peptide
ring and intercalate at sites two base pairs apart; the peptide ring
seems to fit into the minor groove of the DNA. The quinoxalines echinomycin (= quinomycin A) and triostin A differ only
in the nature of the cross-bridge; both show some preference
for GC-rich natural DNAs. TANDEM (des-N-tetramethyltriostin
A: a synthetic analogue of triostin A) shows a marked preference for AT-rich sequences. Quinoxalines are antimicrobial and
antitumour agents; they inhibit the chain elongation stage of
DNA-directed RNA synthesis.
Quinqueloculina See FORAMINIFERIDA.
quinsy Peritonsillar ABSCESS (usually due to Streptococcus pyogenes) a complication of TONSILLITIS.
quintozene (PCNB)
Pentachloronitrobenzene, an agricultural
antifungal agent used mainly for the treatment of soil; it is
effective against a number of soil- and seed-borne diseases,
e.g. DAMPING OFF, various rots of bulbs. Quintozene is insoluble
in water and is used as a dust; it is very stable and has low
volatility hence it is very persistent in the soil. (cf. TECNAZENE,
DICLORAN.)
quinupristin/dalfopristin (RP 59500; Synercid ) A bactericidal
antibiotic (within the STREPTOGRAMIN group) which is active
against e.g. most streptococci (including S. pneumoniae), MRSA,
and Enterococcus faecium (E. faecalis is resistant); it has a
long POST-ANTIBIOTIC EFFECT [Drugs (1996) 51 (supplement 1)
3137]. [In vitro activity against Staphylococcus aureus: JAC
(1997) 39 5358.]
Quinupristin/dalfopristin (administered intravenously) has
been conditionally licenced in Europe and the USA; it has been
useful e.g. for treating vancomycin-resistant infections. Sideeffects include arthralgia and myalgia.
[Quinupristin/dalfopristin (when to use?): JAC (2000) 46
347350.]
qundai-cai See UNDARIA.
quorum sensing The phenomenon in which cells express particular characteristic(s) only when present as a population whose
density is above a certain minimum (quorum). (Here, the density of a population refers to the number of cells per unit
volume.) Thus, in some cases, cells in a high-density population
exhibit characteristics which are absent when the same cells are
in a low-density population.
One example of quorum sensing is that of Photobacterium
fischeri (sometimes referred to as Vibrio fischeri ). P. fischeri
can occur either as a free-living organism (in low-density
populations), or as a symbiont in high-density populations within
the light-emitting organs of certain fish; as a symbiont, P. fischeri
produces a blue-green BIOLUMINESCENCE whereas in the freeliving state (low-density population) it produces little or no light.
OH
O
CH3O
CH3
CH3O
(a)
+2e, +2H
2e, 2H
CH3
CH3O
+
+
CH3O
(b)
OH
O
CH3
R
O
(c)
Benzoquinones include plastoquinones (2,3-dimethylbenzoquinones) and ubiquinones (coenzymes Q); the latter are 2,3dimethoxy-5-methyl-1,4-benzoquinones with a variable-length
isoprenoid side-chain at the 6-position. (Ubiquinones are given
various designations based either on the number of isoprenoid
units or on the number of carbon atoms in the side-chain: e.g.,
a ubiquinone with a side-chain containing 8 isoprenoid units
may be designated ubiquinone-8, UQ-8, UQ8 , coenzyme Q8 , or
ubiquinone-40, UQ-40, etc.) [Book ref. 89.]
Naphthoquinones include e.g. various pigments and toxins
(see e.g. NAPHTHAZARINS and XANTHOMEGNIN), as well as the
K vitamins: derivatives of 2-methyl-1,4-naphthoquinone (vitamin K3 , menadione) in which the 3-position may be substituted with a mono-unsaturated phytyl chain (in vitamin K1 , =
phylloquinone) or with a variable-length polyisoprene chain
(in vitamins K2 , = menaquinones). (Menaquinone terminology
resembles that for ubiquinones: hence, e.g., menaquinone-6,
MK-6, MK-30, vitamin K2(30) etc.) Some bacteria (e.g. members of the PASTEURELLACEAE) contain menaquinones which lack
the 2-methyl group (2-demethyl-vitamins K2 ). In mammals, vitamins K are important components of the blood coagulation
system; mammals cannot synthesize these vitamins, depending
on diet (particularly green plants) and on the bacterial flora of
the gut (particularly Escherichia coli and Bacteroides spp) for
an adequate supply.
Quinones can be reversibly reduced to hydroquinones; they
function e.g. in aerobic and anaerobic ELECTRON TRANSPORT
CHAINS, in PHOTOSYNTHESIS, etc. For example, E. coli synthesizes
both ubiquinone-8 and menaquinone-8 in proportions which
depend on growth conditions; the quinones function as carriers
of reducing equivalents between dehydrogenases and terminal
enzyme complexes (cytochrome oxidases, nitrate reductase, or
fumarate reductase) ubiquinone reduction involving the gain
of two electrons followed by the addition of two protons. The
menaquinone is specifically required for FUMARATE RESPIRATION,
and is also required for the anaerobic synthesis of e.g. pyrimidines (linking dihydro-orotate dehydrogenase with fumarate
reductase in the anaerobic synthesis of uracil). (See also QUINOPROTEIN.)
638
quorum sensing
(Bacterial bioluminescence is used by the fish to signal to one
another.)
The mechanism of quorum sensing involves certain secreted
molecules which, only in high-density populations of the secreting cell, reach a threshold concentration which is sufficient to
trigger specific gene(s) within the cells. The secreted signalling
molecule is referred to as an autoinducer because the cells themselves produce it.
Autoinducers are low-molecular-weight molecules. Different
bacteria may produce different types of autoinducer that regulate different characteristics; however, in some cases different
species may produce the same type of autoinducer for regulating different genes. A given species may produce a range of
autoinducers to control the expression of various characteristics.
In many Gram-negative bacteria, the autoinducer is an N acyl-L-homoserine lactone (AHL). [AHL-based quorum sensing:
TIBS (1996) 21 214219.] In general, AHLs appear to act by
diffusing into the cell and binding to an appropriate cytoplasmic
protein involved in regulating the transcription of relevant
gene(s). In the case of P. fischeri, an AHL triggers the lux
operon (see BIOLUMINESCENCE). [Evolution of LuxI and LuxR as
regulatory molecules in quorum sensing: Microbiology (2001)
147 23792387.]
Strain CV026 of Chromobacterium violaceum is an inducernegative mutant which produces VIOLACEIN when exposed to
exogenous inducers, including all tested molecules of AHL
and AHT (N-acylhomocysteine thiolactone) with N-acyl sidechains between C4 and C8 ; this mutant strain can therefore be
used as a biosensor for detecting a range of inducer molecules
[Microbiology (1997) 143 37033711].
In Pseudomonas aeruginosa the genes encoding certain virulence factors are regulated by at least two quorum sensing
systems the las and rhl systems that involve different AHL
autoinducers; these systems appear to act hierarchically, i.e.
one system is always activated before the other [TIM (1997)
5 132134]. The product of gene qscR appears to be a negative
regulator of quorum-sensing-controlled genes; it probably acts
by repressing gene lasI (which encodes N-3-(oxododecanoyl)
homoserine lactone) [PNAS (2001) 98 27522757].
Quorum sensing has been reported to regulate expression of
the type III PROTEIN SECRETION system in both EHEC and EPEC
strains of Escherichia coli this involving induction of genes in
the LEE PATHOGENICITY ISLAND; regulation of the LEE operons
involves an autoinducer encoded by gene luxS. To account
for the unusually low infectious dose (low-density population)
of E. coli O157:H7, it has been suggested that inducer may
639
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
R
only moderately immunogenic and is apparently not associated
with virulence. It occurs in two antigenically distinct forms: R28
(trypsin-resistant) and R3 (trypsin-sensitive). (See also M PROTEIN
and T PROTEIN.)
R strain See SMOOTHROUGH VARIATION.
r-strand (in adenoviruses) See ADENOVIRIDAE.
R-TEM b-lactamase Syn. TEM-1 b-LACTAMASE.
R1 plasmid A low-COPY NUMBER, IncFII CONJUGATIVE PLASMID
(MWt ca. 60000) which occurs in enterobacteria; it encodes
resistance to e.g. ampicillin, chloramphenicol, sulphonamides
and streptomycin. Replication is promoted, at the origin, by
the (plasmid-encoded) RepA protein, and the frequency of
plasmid replication is controlled by the regulation of RepA
synthesis. The main negative control exerted on RepA synthesis
is carried out by the copA product, an unstable, constitutively
produced micRNA (see ANTISENSE RNA), of half-life ca. 12
minutes, which binds to the complementary sequence (copT )
on the repA mRNA, thus inhibiting translation of the RepA
protein; the inhibitory influence of the copA/copT system
decreases with decrease in copy number thereby providing a
mechanism for stabilizing copy number. (CopA also has a role
in INCOMPATIBILITY in IncFII plasmids.) It has been proposed
that the level of repA expression is also affected by a region
(designated 7k ) within the repA leader sequence; translation of
(i.e., the presence of ribosomes in) this region, which overlaps
the copT sequence, is believed to counteract the negative control
of the copA/copT system [EMBO (1987) 6 515522].
R6 plasmid An enterobacterial IncFII CONJUGATIVE PLASMID
(COPY NUMBER: 12); it encodes resistance to e.g. chloramphenicol, streptomycin, sulphonamides and mercury.
R6K plasmid A multicopy enterobacterial CONJUGATIVE PLASMID
(ca. 38 kb) which carries genes specifying resistance to ampicillin and streptomycin. R6K apparently undergoes sequential
bidirectional replication from any of three origins (designated
a, b and g), all of which are located within a 4-kb region of
the plasmid. Replication initiated at an origin apparently proceeds first in one direction, stopping at a specific termination
site (ter ); re-initiation then occurs at the same origin and proceeds in the opposite direction to ter, thus completing replication
of the plasmid.
Initiation of replication at any of the three origins requires
a trans-acting R6K-encoded DNA-binding protein (the p or
Pi protein) and a region within the g-origin containing seven
tandemly-arranged 22-bp direct repeats (ITERONS). Plasmids from
which the g-origin has been deleted cannot be replicated even
when p is supplied in trans; the a- and b-origins each appear
to have a minimum functional size of ca. 2 kb which includes
the seven iterons in the region of the g-origin. (Deletion
of three or more of the iterons results in loss of plasmid
replicability.) The p protein binds preferentially to the iterons
and positively regulates initiation of replication from one of
the origins (a, b or g). At high concentrations, p can also
play a role in the negative regulation of R6K replication,
apparently by specifically repressing replication from the g
origin. (Experiments involving variation in the levels of p over
a wide range suggest that the level of p in the cell is not
responsible for controlling the copy number of R6K.)
The p protein can also bind to the promoteroperator region
of its own gene (pir, located near the g origin); this region
(1) RONTGEN
(q.v.). (2) (in cell cycle) See CELL CYCLE.
(3) Arginine (see AMINO ACIDS).
R antigen (streptococcal) Syn. R PROTEIN.
R body A refractile, intracellular structure which occurs e.g.
in certain bacterial endosymbionts of protozoa (see CAEDIBACTER) and which appears to confer killer characteristics on the
protozoan host cell. An R body consists of a proteinaceous ribbon, ca. 0.20.5 m wide and ca. 1015 m in length, which
is rolled up to form a cylinder; under negative phase-contrast
MICROSCOPY it appears as a bright ring or (when viewed in
section from the side) as a pair of parallel rods. Its presence
within a bacterial cell is apparently associated with the presence
of plasmid(s) and/or phage(s). R bodies appear to unroll in the
food vacuoles of sensitive paramecia; unrolling appears to occur
from the inside or outside of the coil according to the species of
the bacterium of origin.
R bodies have also been found in free-living strains of
Pseudomonas which are toxic for sensitive paramecia [Arch.
Micro. (1979) 121 915] and in a free-living Pseudomonas-like
bacterium [JGM (1986) 132 28012805].
r-chromatin Chromatin containing rRNA genes.
R factor (1) See R PLASMID. (2) Release factor: see PROTEIN
SYNTHESIS.
R-glucan Alkali-resistant (i.e. alkali-insoluble) glucans of fungal
CELL WALLS.
R loop (mol. biol.) A single-stranded loop of DNA formed
when a short ssRNA molecule pairs with a complementary
region of one strand of a dsDNA molecule, displacing the
corresponding region of the homologous strand (the R loop).
An R loop can be observed by electron microscopy using
the KLEINSCHMIDT MONOLAYER TECHNIQUE. If the ssRNA used
is a mature mRNA derived from a SPLIT GENE, an intron in
the DNA having no homologous region in the mRNA will
appear as a loop of dsDNA extruded between two R loops (each
R loop corresponding to one of the two adjacent exons); thus,
R-looping can be used e.g. to detect introns in genes. (cf. D
LOOP.)
r plasmid See R PLASMID.
R plasmid (formerly R factor, drug resistance factor etc)
Any
PLASMID which encodes resistance to one or more ANTIBIOTICS
and/or to other antimicrobial agents (including e.g. heavy metal
ions). A bacterium containing an R plasmid may express
resistance e.g. by synthesizing a (plasmid-encoded) enzyme which
destroys/modifies an antibiotic (see e.g. CHLORAMPHENICOL, bLACTAMASES) or which modifies the target site (see e.g. MLS
ANTIBIOTICS), or by synthesizing a drug-resistant form of a target
enzyme (see e.g. SULPHONAMIDES).
A conjugative (= transmissible) R plasmid also contains
genes which specify the intercellular transfer of the plasmid
by CONJUGATION (sense 1b) (see also RTF); a non-conjugative
(= non-transmissible) R plasmid does not specify its own
conjugal transfer but it may be mobilized by a conjugative
plasmid. (Some authors refer to a non-conjugative R plasmid as
an r plasmid.) R plasmids belong to various Inc groups (see
INCOMPATIBILITY).
R point (in cell cycle) See CELL CYCLE.
r-protein Ribosomal protein: see RIBOSOME.
R protein (R antigen) (in streptococci) A cell-surface protein
found in streptococci of groups A, B, C and G. R protein is
640
radiolaria
In cattle and horses, symptoms are variable. In vampire bats
(important reservoirs of infection in Central and South America) only the dumb form occurs. Vaccines for use in animals
may be live attenuated (see e.g. FLURY VIRUS) or inactivated. (cf.
AUJESZKYS DISEASE.)
rac prophage See RECF PATHWAY.
race (1) (mycol.) PHYSIOLOGICAL RACE. (2) A non-specific designation which may refer e.g. to a STRAIN or a VARIETY.
racket mycelium Syn. RACQUET MYCELIUM.
racquet mycelium (racket mycelium) In DERMATOPHYTES: mycelium composed of hyphal cells which have terminal swellings
and which thus resemble long-handled tennis racquets.
rad Radiation absorbed dose: a unit of absorbed radiation equal
to 100 ergs of energy absorbed by 1 g of material (0.01 joules
absorbed by 1 kg). (See also GRAY and IONIZING RADIATION; cf.
RONTGEN
.)
RadA protein In members of the Archaea: a protein apparently analogous to the bacterial RecA protein [GD (1998) 12
12481253].
radappertization Irradiation of food with levels of IONIZING
RADIATION sufficient to inactivate the spores of Clostridium
botulinum. (cf. RADICIDATION; RADURIZATION.)
Radar See PROPICONAZOLE.
radiation (in disinfection and sterilization) See IONIZING RADIATION; MICROWAVE RADIATION; ULTRAVIOLET RADIATION.
radicidation Irradiation of food with levels of IONIZING RADIATION sufficient to inactivate certain non-sporing pathogens (e.g.
Salmonella spp). (cf. RADURIZATION; RADAPPERTIZATION.)
radioallergosorbent test See RAST.
radioautography Syn. AUTORADIOGRAPHY.
radioimmunoassay (RIA) A highly sensitive IMMUNOASSAY by
which antigens or antibodies are quantified using radioactive
labelling.
Antibody assay. Essentially, the antiserum under test is
allowed to react with excess homologous antigen (radiolabelled
e.g. with 125 I), and the immune complex is separated from any
uncombined antigen e.g. by precipitation (as in the FARR TECHNIQUE); the amount of antigen in the immune complex is then
determined from the level of radioactivity in the complex, and
the amount of antibody can hence be calculated.
Antigen assay. This is based on the fact that the proportion of
a fixed amount of radiolabelled antigen which combines with a
fixed amount of homologous antibody depends on the amount of
unlabelled antigen present: the more unlabelled antigen present,
the smaller the proportion of labelled antigen and the lower
the level of radioactivity in the immune complex. Thus it
is possible to construct a standard curve for the amount of
unlabelled antigen corresponding to given levels of radioactivity
in the immune complex. In antigen assays, the antigen to be
quantified is the unlabelled antigen, the amount of which can
be derived from the standard curve. (cf. IMMUNORADIOMETRIC
ASSAY.)
radioimmunosorbent test See RIST.
radiolaria A group of free-living, marine, mostly planktonic
protozoa (superclass ACTINOPODA) in which the cells are typically
more or less spherical (<100 m to several millimetres in
diameter) or thimble-shaped, and are generally solitary, although
some species form aggregates or colonies up to 10 cm or more
across. Most radiolaria have a siliceous skeleton consisting
of a delicate internal latticed shell and/or an array of radiating
spines. The cell characteristically contains a central capsule: a
spherical membranous structure, concentric with the cell, which
separates the ectoplasm (extracapsular zone) from the endoplasm
radiolarian ooze
Raffinose is second to sucrose as the most abundant free
sugar in plants. It can be metabolized by many yeasts and fungi
and by certain bacteria; the ability to ferment raffinose is used
to distinguish between top- and bottom-fermenting strains of
BREWERS YEAST.
ragi A type of STARTER culture made in Asian countries by
growing mould(s) on cakes of rice or wheat flour. A ragi is used
as an inoculum in the preparation of various foods, and may
contain e.g. species of Mucor, Rhizopus, Neurospora, various
yeasts etc. (cf. ONCOM; KOJI.)
Rahnella A genus of bacteria of the ENTEROBACTERIACEAE, found
in fresh water and occasionally in human clinical specimens.
Cells are motile when grown at 25 C, non-motile at 36 C. VP
+ve; MR usually +ve. [Book ref. 22, p. 513.]
Ralfsia See PHAEOPHYTA.
Ramalina A genus of fruticose LICHENS (order LECANORALES).
Thallus: strap-like (but not dorsiventral) and erect or pendulous,
attached to the substratum by a discoid holdfast. Apothecia:
terminal and/or marginal. Species occur in unpolluted regions
e.g. on coastal rocks (R. polymorpha, R. siliquosa) or on treebark (R. farinacea, R. fastigiata, R. fraxinea).
Ramibacterium ramosum See CLOSTRIDIUM (C. ramosum).
Ramon titration A serological titration in which a constant
volume of a given antigen solution is added to each of a number
of serial dilutions of homologous antiserum; precipitation occurs
most rapidly in that dilution in which antibody and antigen are
present in OPTIMAL PROPORTIONS.
Ramsay Hunt syndrome HERPES ZOSTER affecting the facial
nerve, causing pain in the ear and face.
Ramularia See HYPHOMYCETES.
ramus A branch. (See also PENICILLIUM.)
Ranavirus A genus of viruses (family IRIDOVIRIDAE) which infect
amphibians. Type species: FROG VIRUS 3.
rancidity In certain lipid-containing foods: a form of spoilage
characterized by the presence of organoleptically detectable
amounts of the products of lipid autoxidation (see OXIDATIVE
RANCIDITY) and/or of the products of the microbial hydrolysis of
lipids (see e.g. BUTTER, CHEESE SPOILAGE).
random amplified polymorphic DNA See RAPD.
random coil See HELIXCOIL TRANSITION.
random walk A pattern of motility, exhibited e.g. by (peritrichously flagellated) enterobacteria, in which periods of smooth
swimming are interrupted by episodes of tumbling (see FLAGELLAR MOTILITY for mechanism); tumbling causes a cell to adopt
a new direction entirely at random, so that in a uniform environment cells move (walk) randomly in three dimensions.
Although tumbling results in a random change of direction, a
cell can nevertheless bias the net direction of its motility in
response to certain directional stimuli (see TAXIS) by increasing or decreasing the frequency of tumbling when travelling in
(respectively) an unfavourable or favourable direction. During
CHEMOTAXIS, for example, cells of e.g. Escherichia coli which
encounter an unfavourable gradient of nutrients increase their
frequency of tumbling thus reducing the time they swim in
an unfavourable direction; conversely, the tumbling response is
repressed if a more favourable location is encountered, and a
longer period of smooth swimming supervenes. Thus, there is a
net movement towards a favourable stimulus and away from an
unfavourable one a type of tactic response known as a biased
random walk.
Ranikhet disease Syn. NEWCASTLE DISEASE.
RANTES (chemokine) See CHEMOKINES.
RapA phosphatase See ENDOSPORE (sense 1).
reaction centre
bound IgE is detected by the addition of radiolabelled anti-IgE
antibodies.
rat-bite fever Either of two human diseases contracted from
the bite of a rat or, less commonly, a cat, dog etc. One form
(Haverhill fever) is caused by Streptobacillus moniliformis;
symptoms include e.g. the development of a fluid-filled sore at
the site of the bite, a skin rash, recurrent fever, lymphadenopathy,
and more or less generalized arthritis. The second form (sodoku)
occurs more commonly in Japan and other Eastern countries
and is caused by Spirillum minus (see SPIRILLUM); symptoms
resemble those of Haverhill fever, but there is usually no
arthritis.
rat leukaemia viruses Ecotropic type C retroviruses (subfamily
ONCOVIRINAE) which are apparently ubiquitous in rats; none is
known to be leukaemogenic or to have any oncogenic potential.
[Book ref. 114, pp. 101104.]
rat virus See PARVOVIRUS.
ratezonal centrifugation See CENTRIFUGATION.
Ratkowsky plot The square root of growth rate plotted against
absolute temperature; in various bacteria, this plot shows a
linear relationship over the full biokinetic range [JB (1983) 154
12221226].
Rauscher virus (RV) A virus complex consisting of at least two
components: a replication-competent MURINE LEUKAEMIA VIRUS
(Ra-MuLV) and a replication-defective SFFV (cf. FRIEND VIRUS);
within ca. 14 days of infection of newborn or adult mice, RV
induces splenomegaly and anaemia (erythroblastosis), followed
after several weeks by the onset of lymphocytic leukaemia.
raw water See WATER SUPPLIES.
ray body (Strahlenkorper) A microgamont or an isogamete of
Babesia or Theileria.
ray fungus Archaic term for an ACTINOMYCETE.
razor-strop fungus Piptoporus betulinus.
RB Reticulate body (see CHLAMYDIA).
RBC Red blood cell (erythrocyte).
Rc strain See SMOOTHROUGH VARIATION.
RCF (relative centrifugal field) See CENTRIFUGATION.
RCM REINFORCED CLOSTRIDIAL MEDIUM.
Rd1 strain See SMOOTHROUGH VARIATION.
Rd2 strain See SMOOTHROUGH VARIATION.
RD-114 viruses See FELINE LEUKAEMIA VIRUS.
RDE RECEPTOR-DESTROYING ENZYME.
rDNA DNA coding for rRNA.
RE RESTRICTION ENDONUCLEASE.
Re strain See SMOOTHROUGH VARIATION
REA See DNA FINGERPRINTING.
reaction centre In photosynthetic membranes: a type of pigmentcontaining complex, distinct from LIGHT-HARVESTING COMPLEXes,
to which radiant energy is channelled and at which charge
separation occurs (see PHOTOSYNTHESIS).
In algae and cyanobacteria, the photosynthetic membranes
contain two types of reaction centre (RC). The RC in photosystem I includes a specialized form of CHLOROPHYLL a designated
P700 (indicating its absorption maximum of 700 nm); the RC
chlorophyll represents only ca. 1/300th of the chlorophyll content of the membrane. The RC of photosystem II also appears to
contain a chlorophyll a moiety (designated P680 again, to indicate its absorption maximum) together with e.g. phaeophytin a.
The RCs of several anoxygenic photosynthetic bacteria
have been characterized. Thus, e.g. that in Rhodopseudomonas
sphaeroides includes bacteriochlorophyll a (P870 ), bacteriophaeophytin a, ubiquinone and ferrous iron; the RC in R. viridis
includes bacteriochlorophyll b, bacteriophaeophytin b, and
reactivation
161165], Bacillus subtilis [JBC (1985) 260 33053313],
Methylophilus methylotrophus [Gene (1986) 44 4753], Vibrio cholerae [MGG (1986) 203 5863], and Ustilago maydis
(the rec1 gene product) [Cell (1982) 29 367374].) In members of the Archaea, the RadA protein is homologous to RecA
[GD (1998) 12 12481253].
The RecA protein plays an essential role in general RECOMBINATION, and can promote various interactions between DNA
molecules (including synapsis, strand exchange and branch
migration) provided that at least one of the DNA molecules is
at least partly single-stranded. For example, in vitro, RecA can
promote base-pairing between a ccc ssDNA molecule and its
complementary strand in a (linear) dsDNA molecule; the ssDNA
invades the dsDNA molecule and displaces the homologous
strand (a phenomenon known e.g. as single-strand assimilation). This reaction is initiated when RecA binds stoichiometrically and cooperatively to ssDNA in the presence of ATP to
form a helical nucleoprotein filament [structure: JMB (1986)
191 677697] (presynaptic stage); polymerization is accelerated
in the presence of SINGLE-STRAND BINDING PROTEIN (SSB protein) and is inhibited by ADP. The RecAssDNA complex then
interacts with dsDNA to form a ternary dsDNAssDNARecA
complex in which the dsDNA becomes extensively unwound.
The ternary complex can be formed in the absence of homology;
it is generally believed that a search for homology between the
ssDNA and dsDNA must then occur. Juxtaposition of complementary regions (synapsis) results in the formation of a nascent
heteroduplex joint. Recent studies suggest that (contrary to an
earlier view) the search for homology is unlikely to involve
a triplex DNA intermediate but may involve unwinding of
the target duplex coupled with local strand exchange; it also
appears that the polarity of RecAssDNA does not affect its
ability to interact with a circular target duplex [NAR (2001) 29
13891398].
RecA-promoted strand exchange can continue through regions
of mismatched bases, past thymine dimers, and past deletions or
insertions in one of the strands.
The single-strand assimilation reaction per se is probably of
limited significance in vivo (cf. TRANSFORMATION). However, in
vitro, the RecA protein can also promote pairing between two
dsDNA molecules provided that there is a gap in one of them,
a reaction which may resemble more closely a homologous
recombination event in vivo; the necessary regions of ssDNA
may be provided e.g. by the RECBC PATHWAY.
[Role of RecA in recombination: CSHSQB (1984) 49
507580; mechanistic aspects of DNA strand exchange activity
of RecA: TIBS (1987) 12 141145.]
The RecA protein is normally synthesized at a low level
in the cell, being repressed to this level by the product of
the lexA gene. However, under certain conditions e.g. in
the presence of damaged DNA the RecA protein becomes
activated, acquiring the ability to trigger proteolytic cleavage
of the LexA protein (thus inducing the SOS SYSTEM q.v.) and
of the repressor proteins of BACTERIOPHAGE LAMBDA and other
LAMBDOID PHAGES (thus initiating prophage induction).
RecA See SOS SYSTEM.
recapitulation theory See ONTOGENY.
recB gene See RECBC PATHWAY.
RecBC pathway A pathway for general RECOMBINATION in
Escherichia coli and related bacteria; it appears to be the major
pathway for recombination following CONJUGATION. The pathway
requires the products of the recA gene (see RECA PROTEIN) and of
the recB and recC genes, the latter two being components of a
recombination
multifunctional enzyme formerly known as the RecBC enzyme
or exonuclease V. More recently, this enzyme (330 kDa) has
been re-designated the RecBCD enzyme.
The RecBCD enzyme carries out functions in one of two
major pathways (recombination machines) for homologous
recombination in Escherichia coli. In this pathway the enzyme
is responsible e.g. for repairing double-stranded breaks in DNA;
repairs can be carried out only on linear substrates including
circular molecules with a double-stranded break.
The RecBCD enzyme has helicase and nuclease activities,
and it also has a synaptogenic function (see later). One of the
differences between the RecBCD pathway and the RecF pathway
is that the former involves a single, multi-subunit enzyme while
the latter involves the activities of a number of separate enzymes.
As in the RecF pathway, recombination can be initiated
in the RecBCD pathway; in RecF, initiation is triggered e.g.
by a single-stranded gap in the chromosome, while in the
RecBCD pathway initiation is prompted e.g. by DNA damage
involving a double-stranded break. Given a double-stranded
break, the (ATP-dependent) RecBCD nuclease may degrade a 5
terminal, leaving a free (single-stranded) 3 terminal to which
molecules of the RecA protein bind, forming the nucleoprotein
filament. (RecBCD mediates the exclusion of single-strand
binding proteins from the 3 terminal; this is necessary in order
to permit binding of RecA monomers.)
A nucleoprotein filament is apparently the initial structure
formed in all cases of homologous recombination (including
recombination mediated by RecBCD and RecF systems).
The nucleoprotein filament is believed to search another
(target) duplex for a sequence of nuleotides homologous to the
sequence in the nucleoprotein itself. This may involve local
unwinding of the target duplex. The juxtaposition of homologous
sequences (synapsis) leads to the formation of a hybrid duplex
(heteroduplex). Events may then proceed as described for the
Holliday model: see RECOMBINATION.
Recombination via the RecBCD pathway is stimulated by
the presence of certain sequences of nucleotides within the
chromosomal DNA. For example, the E. coli chromosome has
about 1000 copies of the sequence:
5 GCTGGTGG3
i.e. about one copy per 5 kb of DNA; these sequences, which
are called chi (c) sites, enhance homologous recombination in
their vicinity.
The RecBCD enzyme has an affinity for chi sites and, as a
result of interaction between RecBCD and a chi site, a chi site
tends to be found at or near the 3 terminus of DNA in the
nucleoprotein filament.
Chi-dependent activity has been reported in other enterobacteria, and e.g. in some species of the family Vibrionaceae, but
appears to be absent in various other bacteria; it may be that
different sequences of nucleotides play a similar role in other
types of bacteria.
More recently it has been found that certain functions of
the RecBCD and RecF pathways are interchangeable; if, for
example, a null mutation occurs in the recD (nuclease) subunit
of RecBCD then this function can be compensated for by the
RecJ nuclease of the RecF pathway. [Interchangeable parts of
the Escherichia coli recombination machinery: Cell (2003) 112
741744.]
recC gene See RECBC PATHWAY.
recE gene See RECF PATHWAY.
RecE pathway See RECF PATHWAY.
645
(f)
(a)
(b)
x
(g)
(c)
(h)
(d)
(e)
(i)
RECOMBINATION: Figure 1. Holliday model [Genet. Res. (1964) 5 282304]. (a) Two homologous DNA duplexes; the 3 ends are identified by
arrowheads. (b) A nick occurs at corresponding sites in one strand of each duplex. (c) One strand from each duplex begins to pair with the
complementary strand of the other duplex to form a heteroduplex joint. (d) Ligation results in a branched half-chiasma (a Holliday structure or
Holliday junction); the position of the branch may move (branch migration) in either direction and may increase the length of the heteroduplex
region (as shown). Resolution of the Holliday structure by nicking, exchange and re-ligation of the crossed strands results in the molecule
shown at (e); in this case markers flanking the heteroduplex region are not exchanged (i.e., there is no CROSSING OVER). (f) Unstacking of the
bases at the site of the joint allows the formation of a symmetrical chi structure which can undergo the isomerizations shown at (g) and (h):
rotation through 180 of the two lower arms about axis y gives the structure at (g), and a subsequent 180 rotation of the two right-hand
arms about axis x gives the structure at (h). This results in the crossing of the previously un-nicked (outer) strands; resolution of the Holliday
structure by nicking, exchange and ligation of these strands results in reciprocal exchange of flanking markers (crossing over) to give the
recombinant duplexes shown at (i).
646
(a)
(a)
(b)
(b)
(c)
(c)
(d)
(d)
(e)
(e)
Y
X
(f)
X
Y
(f)
OR
OR
(g)
(g)
RECOMBINATION: Figure 2. A. MeselsonRadding model (Aviemore model) [PNAS (1975) 72 358361]. (a) Recombination is initiated by a
nick in one strand of one of the two homologous duplexes (the donor duplex). (All 3 ends are identified by arrowheads.) (b) The 3 end
generated by the nick serves as a primer for DNA synthesis and is extended (shaded portion), displacing the 5 end which then invades a
homologous region of the other (recipient) duplex to generate a D LOOP. (c) The donor strand is ligated in place, and the D loop is degraded.
(d) The heteroduplex region can be extended by further nuclease action on the recipient duplex and DNA polymerase action on the donor
duplex. Ligation completes the Holliday structure. (e) Branch migration may occur (e.g. as shown). Resolution of the Holliday structure may
occur by exchange between the inner strands, with no crossing over (f), or following isomerization (see Fig. 1) between the outer strands,
resulting in crossing over (g).
B. Double-strand break repair model [Cell (1983) 33 2535]. (a) Recombination is initiated by nicks in both strands of one of the two
homologous duplexes (the recipient duplex). (b) The nicks are enlarged to gaps by exonuclease action, and (c) a free 3 end thus generated
invades a homologous region of the donor duplex, giving rise to a D loop. (d) Extension of the 3 end of the invading strand by repair
synthesis enlarges the D loop until a sequence homologous to the second recipient fragment is exposed. (e) Further repair synthesis and
ligation complete two Holliday junctions; branch migration may occur (not shown). Cutting and ligation at x and X, as in (f), or at y and Y (not
shown) resolve the Holliday structures without crossing over; cutting and ligation at X and y, as in (g), or at x and Y (not shown), result in
crossing over.
647
recombination frequency
alleles (e.g. one wild-type, one mutant) the heteroduplex will
have a region of mispaired bases at the mutation site. Such
mismatched regions may be recognized by a MISMATCH REPAIR
system in which nucleotides are removed from one of the
strands and replaced, by repair synthesis, using the other strand
as template; thus, the nucleotide sequence of one strand is
converted to a sequence complementary to that of the template,
a phenomenon known as gene conversion (an example of nonreciprocal recombination). (In a bacterial merozygote, the term
gene conversion may be restricted to cases in which a sequence
in the recipients DNA is converted to a sequence of the donor
fragment.) Extensive mismatch repair within a long region of
heteroduplex DNA can lead to the conversion of two or more
adjacent alleles (co-conversion). (cf. INTERFERENCE (sense 2) and
POST-MEIOTIC SEGREGATION.)
Although it was originally thought that general recombination could occur with equal probability between any regions
of homology of a given length, it has been found that certain nucleotide sequences (recombinators or recombinogenic
sequences) can specifically enhance general recombination in
their vicinity: see e.g. chi site under RECBC PATHWAY.
In prokaryotes, general recombination may occur e.g. between
donor and recipient DNA in a MEROZYGOTE, between homologous regions of different plasmids or of a plasmid and the
chromosome, etc; in Escherichia coli, at least, several possible pathways of general recombination are known, all of which
apparently require the product of the recA gene (see RECA PROTEIN and e.g RECBC PATHWAY).
In species of the domain ARCHAEA the RadA protein appears
to be equivalent, in function, to the RecA protein.
In viruses, general recombination may occur e.g. between
genomes of viruses that are co-infecting the same cell (cf.
REASSORTANT VIRUS). In certain bacteriophages recombination is
apparently an essential step in the viral replication cycle (see
e.g. BACTERIOPHAGE T4).
In eukaryotes, general recombination may occur in meiosis and occasionally in mitosis: see PARASEXUAL PROCESSES.
recombination frequency Following general RECOMBINATION
(e.g. after meiosis): the number of recombinant progeny, in
respect of the alleles of two different genes, as a proportion
of the total progeny (expressed as a percentage). Recombination
frequency (RF) gives an indication of the relative positions of
markers (genes or mutations) in the genome. An RF of 50% indicates that the markers segregate independently between progeny,
e.g., they occur on different chromosomes; lower frequencies
indicate that the markers occur on the same chromosome the
lower the frequency, the smaller the distance between them. (See
also INTERFERENCE (sense 2) and RECOMBINATOR.)
recombination nodule See SYNAPTONEMAL COMPLEX.
recombination repair In e.g. Escherichia coli : a recA-dependent
DNA REPAIR process which can repair e.g. thymine dimers or
double-strand breaks. During replication of a dsDNA molecule
containing e.g. a thymine dimer, the DNA polymerase stops at
the site of the dimer; DNA synthesis may be re-initiated by
primer synthesis at a site beyond the lesion, leaving a gap in the
daughter strand opposite the dimer in the damaged parent strand.
This gap can be filled by RECOMBINATION between the gapped
daughter strand and an undamaged homologous region of the
strand complementary to the damaged parent strand (daughterstrand gap repair ). The resulting gap in the homologous parent
strand can then be filled by repair synthesis, its daughter strand
acting as template. The dimer is thus not removed, but is
effectively diluted out. Genes apparently involved in daughterstrand gap repair include recA, ruv, lexA and recF ; levels
redox potential
red rice Syn. ANG-KAK.
red rot (1) A SUGARCANE DISEASE caused by Colletotrichum
falcatum; fungal attack is generally concentrated within the stem
and midribs of the leaves, with reddening of internal tissues and
withering of the tips and margins of the leaves.
(2) See ALGAL DISEASES.
red rust (algal rust) A disease of tea (Camellia sinensis) and various other commercially important plants (e.g. avocado, cacao,
citrus, coffee, mango) caused by a species of CEPHALEUROS. The
alga grows beneath the cuticle of the leaves and stems, resulting
in the formation of elevated, velvety, reddish or orange-brown
lesions. Infected leaves may exhibit a wound response, with
necrosis of tissue around the lesions, which may help to prevent
the spread of the alga. Infections of leaves and fruit generally
cause little harm to the plant, apart from the unsightly lesions
and in heavily infected plants premature leaf-drop. However, infections of young stems may be more serious, and plants
may even be killed if the stems are completely girdled. [Review:
Book ref. 129, pp. 173204.] The disease has been controlled
with copper sprays. (See also BLISTER BLIGHT.)
red snow In mountainous areas of western North America:
snow which appears reddish owing to the abundant growth
of Chlamydomonas nivalis, C. nivalis grows in spring and
summer mainly near the surface of the melting snow; it forms
the basis of a fairly extensive food-chain involving protozoa,
rotifers, nematodes and crustaceans.
red tide (red water) A phenomenon in which regions of the sea
or of an estuary become discoloured (often red or reddish) owing
to extensive BLOOMS of certain algae particularly DINOFLAGELLATES. (Blooms of the cyanobacterium TRICHODESMIUM are sometimes called red tides.) For example, Gonyaulax catenella and
G. tamarensis (= e.g. G. excavata, Protogonyaulax tamarensis,
Alexandrium tamarense) are common causes of red tides on
the coasts of North America, while Ptychodiscus brevis (=
Gymnodinium breve) forms red tides in the Gulf of Mexico and
along the Florida coast. Blooms of G. tamarensis are seasonal;
evidence has been obtained for the existence of an endogenous
annual clock (circannual rhythm) in G. tamarensis from deep
coastal waters [Nature (1987) 325 616617].
A red tide can cause massive mortalities in fish and other
aquatic animals due to oxygen depletion and/or to the production of various toxins (e.g. BREVETOXINS, GONYAUTOXINS,
SAXITOXIN). These toxins can also cause poisoning in man, particularly when shellfish from affected waters are eaten (see
paralytic SHELLFISH POISONING).
red vent disease Syn. ENTERIC REDMOUTH.
red wasting disease See ALGAL DISEASES.
red water (1) (of calves) An acute, febrile, often fatal disease of
young calves, characterized by jaundice and haemoglobinuria;
it is caused by Leptospira interrogans serotype pomona (cf.
LEPTOSPIROSIS).
(2) Any of various diseases characterized by haemoglobinuria.
(See also REDWATER FEVER.)
(3) Syn. RED TIDE.
red water fever See REDWATER FEVER.
redox couple See REDOX POTENTIAL.
redox dye See REDOX POTENTIAL.
redox potential (oxidationreduction potential; Eh ; E) A measure of the tendency of a given system to donate electrons (i.e.,
to act as a reducing agent) or to accept electrons (i.e., to act as
an oxidizing agent); the Eh of a given system may be determined
e.g. by measuring the electrical potential difference between that
system and a standard hydrogen electrode whose potential is,
reduction division
Certain dyes (redox dyes, or indicators) can indicate Eh by
changing from a coloured to a colourless state (and vice versa)
within a given Eh range; thus, e.g. a dye may become completely
colourless (at pH 7) when the Eh is ca. 40 mV (e.g. METHYLENE BLUE), ca. 70 mV (e.g. toluidine blue), ca. 110 mV (e.g.
resazurin), and ca. 310 mV (e.g. phenosafranine). (See also
TETRAZOLIUM.)
Eh of microbiological media. In general, an obligate ANAEROBE can grow only on or in media which are at or below a certain
value of Eh . For this reason media are often poised at a certain
Eh ; poising is analogous to buffering in the context of pH i.e.,
while the Eh produced depends on the ratio oxidized:reduced
poising agent, the stability of Eh is influenced by the absolute
amount of poising agent in the medium. Poising agents used in
media include e.g. ASCORBIC ACID, cysteine hydrochloride and
thioglycollate.
reduction division Syn. MEIOSIS.
reductive carboxylic acid cycle Syn. REDUCTIVE TRICARBOXYLIC
ACID CYCLE.
reductive pentose phosphate cycle Syn. CALVIN CYCLE.
reductive tricarboxylic acid cycle A pathway for CO2 fixation in certain prokaryotic AUTOTROPHS (mainly members of
the Chlorobiaceae cf. SULFOLOBUS). The pathway is effectively the reverse of the TCA CYCLE [see Appendix II],
one molecule of acetyl-CoA being formed for every two
of CO2 fixed; the irreversible steps of the TCA cycle
are bypassed by other enzymes: the 2-oxoglutarate dehydrogenase complex is replaced by 2-oxoglutarate:ferredoxin
oxidoreductase (= 2-oxoglutarate synthase), and citrate synthase by ATP-citrate lyase (citrate + coenzyme A + ATP
oxaloacetate + acetyl-CoA + ADP + Pi). Succinate dehydrogenase is replaced by a (probably NADH-dependent) fumarate
reductase. Acetyl-CoA can be converted to pyruvate (by
ferredoxin-dependent pyruvate synthase) and thence e.g. to
phosphoenolpyruvate which may in turn be carboxylated to
oxaloacetate or used for GLUCONEOGENESIS etc, depending on
the requirements of the cell.
redundant (of genes etc) Present in more than one copy per
chromosome or per genome. (cf. TERMINAL REDUNDANCY.)
redwater fever (murrain; cattle tick fever; Texas fever) An acute,
sometimes fatal disease of cattle and other animals caused by
species of BABESIA; it is transmitted by blood-sucking ixodid
ticks (e.g. species of Boophilus, Dermacentor, Rhipicephalus).
The incubation period is ca. 414 days. Babesia grows within
and destroys the hosts erythrocytes, causing e.g. fever and
haemoglobinuria (hence redwater fever).
ReedMuench method See END-POINT DILUTION ASSAY.
reference strain In bacteriology: any strain which is not a type
strain or a neotype but whose name (or other designation) is
used to define or identify products, antigens etc produced by
that strain.
refractile Refers to structures which appear bright when viewed
by bright-field MICROSCOPY.
refrigeration (of foods) See FOOD PRESERVATION (b).
regulator gene A GENE whose product is a regulator protein
which regulates the transcription of one or more STRUCTURAL
GENES (see e.g. OPERON).
regulon A system in which two or more (usually non-contiguous)
structural genes and/or OPERONS, each with its own promoter,
are subject to coordinated regulation by a common regulator
molecule (e.g., a repressor or activator); the genes/operons share
common or related regulatory sequences (e.g. operators or initiators) which can each be recognized by the regulator molecule.
Reovirus
relaxing enzyme (1) A type I TOPOISOMERASE.
(2) Any enzyme capable of relaxing supercoiled DNA.
relaxosome See CONJUGATION (1b)(i).
release factors (in protein synthesis) See PROTEIN SYNTHESIS (termination).
Relenza See ZANAMIVIR.
relomycin See MACROLIDE ANTIBIOTICS.
Renibacterium
A genus of aerobic, asporogenous, catalasepositive, oxidase-negative bacteria (order ACTINOMYCETALES,
wall type VI); the type species, R. salmoninarum (formerly
Corynebacterium salmoninus) is the causal agent of KIDNEY
DISEASE in salmonid fish. The organisms are rods or coccobacilli,
0.31.0 1.01.5 m, which frequently occur in pairs. Growth
occurs optimally at ca. 1518 C on e.g. cysteineserum agar
(cysteine being required for growth). [Selective isolation of
Renibacterium: FEMS (1983) 17 111114.] GC%: ca. 5354.
reniform Kidney-shaped.
rennet substitutes See PROTEASES.
rennin See CASEIN.
rennin substitutes See PROTEASES.
Reoviridae A family of viruses in which the (non-enveloped)
virion is typically icosahedral or amorphous (6080 nm in
diam.) and contains a segmented genome of 1012 different
linear dsRNA molecules. The virion may contain up to 1013
species of protein; it consists of a core (characteristically a
double-layered structure incorporating the genome) commonly
or always enclosed by an outer capsid layer, the latter being
lost during viral penetration of the host cell. (The outer capsid
layer is generally thought to be important for initial attachment
to the target cell; however, cores of the bluetongue virus from
which the outer capsid layer has been removed are still
infective for the insect vector, even though poorly infective
for mammalian cells [Virology (1996) 217 582593].) The
viral core, released into the cytoplasm of the target cell,
may include e.g. transcriptase, nucleotide phosphohydrolase,
guanylyltransferase and transmethylase enzymes responsible
for synthesis and modification of the viral transcripts. In several
reoviruses
REP sequence (repetitive extragenic palindromic sequence;
palindromic unit) A highly conserved PALINDROMIC SEQUENCE
with hypenated dyad symmetry, ca. 5001000 copies of
which are distributed in the chromosome in e.g. Escherichia
coli, Salmonella typhimurium and other enterobacteria; REP
sequences have also been found in e.g. Listeria monocytogenes.
REP sequences occur between genes, or in the untranslated
promoter-distal region (beyond the genes) in many operons, but
they have not been detected within coding sequences. (See also
ERIC SEQUENCE.)
REP sequences can potentially form cruciform structures in
DNA, or stem-and-loop structures in the corresponding mRNA;
thermodynamically, the latter is more likely.
REP sequences may play a role in nucleoid structure (earlier,
evidence was obtained that REP sequences have protein-binding
sites [FEBS (1986) 206 323328], and they are now known to
be associated with HU PROTEIN).
REP sequences have been used in the typing of bacteria
(by REP-PCR) [e.g. JCM (1999) 37 103109; JCM (1999) 37
27722776].
Repetitive sequences either clustered or dispersed through
the genome have long been recognized in higher eukaryotes:
see e.g. ALU SEQUENCES.
REP1, REP2 genes See TWO-MICRON DNA PLASMID.
repair (of DNA) See DNA REPAIR.
repeating spore (mycol.) A spore from which arises mycelium
of the same type as that from which the spore was formed.
repetitive extragenic palindromic sequence See REP SEQUENCE.
repetitive sequence-based PCR See REP-PCR.
replacement vector A CLONING vector which has a pair of
cleavage sites flanking a dispensable sequence (the stuffer);
the stuffer sequence is removed and replaced by a sequence of
exogenous DNA. (cf. INSERTION VECTOR.)
replica (in microscopy) See ELECTRON MICROSCOPY (a) and (b).
replica plating A technique for isolating mutants from a population of microorganisms grown under non-selective conditions.
For the isolation of e.g. auxotrophic mutants from a population
of prototrophic bacteria, a master plate is prepared by inoculating a plate of complete medium with an inoculum from the
prototrophic population. Following incubation, a disc of sterile
velvet (attached to one end of a cylindrical wooden block) is
pressed lightly onto the surface of the master plate; the disc,
to which has adhered growth from the master plate, is then
used to inoculate one or more plates of minimal medium (the
replica plates) a careful record being made of the orientation
of the disc relative to the master plate and to the replica plates
during inoculation. The replica plates are then incubated; only
prototrophic cells form colonies. The positions of colonies on
the master and replica plates are compared, and presumptive
auxotrophs can be identified by their absence from the replica
plates.
replicase See RNA-DEPENDENT RNA POLYMERASE.
replication fork See DNA REPLICATION.
replicative form See RF.
replicative intermediate See RI.
replicative recombination See TRANSPOSABLE ELEMENT.
replicombinase A TRANSPOSASE which catalyses replicative
recombination (see TRANSPOSABLE ELEMENT).
replicon Any DNA sequence or molecule which possesses a
replication origin and which is therefore potentially capable of
being replicated in a suitable cell (see DNA REPLICATION).
repliconation The process in which a circular dsDNA molecule,
capable of replication, is formed within a cell from DNA that
has been taken up e.g. by CONJUGATION (sense 1b).
R
P
R
P
respiratory burst
in which l is the wavelength of light forming the image,
is the refractive index of the medium between objective and
specimen, and q is half the apical angle of the widest cone of
light which can enter the objective from the specimen plane. The
quantity sin q is the numerical aperture (NA) of the objective;
the higher the NA the better the resolving power. (The NA
of a CONDENSER is also given by sin q; here, q is half the
apical angle of the widest cone of light which can be focused
in the specimen plane.) When the medium between objective
and specimen is air ( = 1.0) the NA is less than 1.0. A greater
NA is obtainable with an immersion lens: a lens designed to
work with a liquid bridge between it and the specimen; an
oil-immersion objective uses IMMERSION OIL ( ca. 1.5), and a
water-immersion objective uses distilled water ( ca. 1.3). The
use of oil or water enables the objective to receive a wider cone
of light from the specimen plane; this increases resolving power
by increasing the amount of diffracted light received from the
specimen (see MICROSCOPY (a)). When using immersion oil, one
drop is placed on the objective lens and another on the coverglass; the objective is racked down until the drops coalesce, and
the specimen is then brought into focus. This method avoids the
risk of trapping air bubbles between lens and cover-glass a risk
greater with objectives that have a concave front lens; air bubbles
cause flare and distortion. Usually, an oil-immersion substage
condenser is used when using an oil-immersion objective lens;
in this case the top lens of the condenser should be oiled to
the underside of the slide in order to obtain maximum resolving
power from the objective lens.
The resolving power of a good light microscope is about
200 nm; with an ultraviolet microscope it is about 130 nm, and
with an electron microscope it can be less than 1 nm.
resorcinol 1,3-Dihydroxybenzene.
resorufin See RESAZURIN TEST.
respiration Energy-yielding metabolism in which the oxidation
of an energy substrate involves an exogenous electron acceptor
(i.e., an externally derived oxidizing agent); the participation
of an exogenous electron acceptor results in the net oxidation
of the energy substrate, and makes possible an energy yield
significantly greater than that obtainable by the fermentation of
the given substrate (cf. FERMENTATION sense 1). Respiration can
occur aerobically or anaerobically (see ANAEROBIC RESPIRATION),
and may involve an inorganic electron acceptor (e.g. oxygen or
nitrate see also NITRATE RESPIRATION) or an organic electron
acceptor (see e.g. FUMARATE RESPIRATION).
In the respiratory (= oxidative) metabolism of an energy
substrate, the exogenous electron acceptor commonly, but not
always, undergoes reduction at the (most positive) end of an
ELECTRON TRANSPORT CHAIN (ETC); electron flow from the substrate, via an ETC, to the electron acceptor typically generates
proton motive force (see CHEMIOSMOSIS) which can be used
for e.g. ATP synthesis (see OXIDATIVE PHOSPHORYLATION). Respiratory metabolism can occur without the involvement of an
electron transport chain, ATP being synthesized entirely by
substrate-level phosphorylation: see e.g. nitrite respiration in
Escherichia coli in entry NITRATE RESPIRATION.
Respiratory substrates include organic compounds (see ORGANOTROPH) and inorganic compounds or ions (see LITHOTROPH);
according to species and conditions, the electron acceptor may
be e.g. oxygen, nitrate, CO2 , sulphate or fumarate. In that the
exogenous electron acceptor is involved in the final oxidative
step in a respiratory pathway it is commonly called the terminal
electron acceptor.
respiratory burst See NEUTROPHIL.
respiratory chain
respiratory chain See ELECTRON TRANSPORT CHAIN.
respiratory control Control of the electron flow in a respiratory
chain by proton motive force (see CHEMIOSMOSIS). According
to its value, pmf may inhibit or promote the further extrusion
of protons across the membrane usually with a concomitant
decrease or increase, respectively, in electron flow. In the socalled State 3 (active state) the rate of respiration is high owing
to decreased pmf; in the presence of UNCOUPLING AGENTS (which
can abolish pmf entirely) respiration is maximal (State 3unc or
3u). In State 4 (the controlled or resting state) respiration is minimal owing to the maximal thermodynamic back-pressure of the
pmf; however, a low level of respiration may occur in order e.g.
to balance the effects of proton leakage across the membrane.
In Escherichia coli the adsorption of certain bacteriophages
has been shown to cause a transient release from respiratory
control, phage adsorption apparently inducing an inflow of
protons similar to that induced by protonophores [JB (1985)
161 179182].
respiratory inhibitors Substances which inhibit the flow of
electrons along a respiratory chain: see e.g. AMYTAL, ANTIMYCIN A,
AZIDE, BAL, CARBON MONOXIDE (b) CYANIDE, DCMU, HYDROXYQUINOLINE-N-OXIDES, PIERICIDIN and ROTENONE. (cf. UNCOUPLING
AGENTS; OLIGOMYCIN.)
respiratory syncytial virus See PNEUMOVIRUS.
respiratory tract microflora The human nasal passages commonly harbour species of Corynebacterium and Staphylococcus
(usually S. epidermidis, sometimes S. aureus also) and occasionally species of e.g. Moraxella and Streptococcus. In the
nasopharynx the predominating organisms are often streptococci; various opportunist pathogens (e.g. Haemophilus influenzae, Streptococcus pneumoniae, strains of Moraxella) may also
be present. (See also MOUTH MICROFLORA.)
The trachea, bronchi, bronchioli and lungs may be sterile
or may have small numbers of contaminating organisms. The
ability of extraneous air-borne particles (see AIR) to reach the
trachea, or to penetrate further into the respiratory tract, is
governed largely by the size and shape of such particles. For
example, spores > ca. 10 m (e.g. those of Alternaria and
Fusarium) tend to be trapped in the nose, but may reach the
bronchi during mouth-breathing; such spores may induce e.g. a
TYPE I REACTION. Spores 510 m (formed e.g. by many species
of Cladosporium and Mucor ) may be deposited in the bronchi
or bronchioles where they may incite attacks of asthma in
susceptible individuals; spores of this size may even penetrate
into the alveoli if an individual is exposed to very large numbers
of spores. Spores < 5 m (e.g. those formed by species of
Aspergillus and Penicillium, and by many actinomycetes) may
reach the alveoli; the spores of actinomycetes are commonly
implicated in certain types of EXTRINSIC ALLERGIC ALVEOLITIS.
(See also BODY MICROFLORA and e.g. BRONCHITIS; COMMON
COLD; CYSTIC FIBROSIS; PNEUMONIA.)
response regulator See TWO-COMPONENT REGULATORY SYSTEM.
resting spore (winter spore) (mycol.) A thick-walled spore, particularly one formed by a sexual process, which germinates only
after an extended period of dormancy e.g. an overwintering
teliospore. (cf. SUMMER SPORE.)
restricted transduction See TRANSDUCTION.
restriction endonuclease (REase, RE; restriction enzyme) An
ENDONUCLEASE which binds to dsDNA, usually at a specific
recognition sequence (= recognition site), and typically makes
a single cut in each strand provided that specific bases at that
site are unmethylated (for some REs) or methylated (for others);
the cleaved duplex may exhibit STICKY ENDS or BLUNT-ENDED
DNA,
restrictionmodification system
RESTRICTION ENDONUCLEASES (REs): some examplesd
RE
Source (organism)
Recognition sequencea
AatII
AluI
ApaI
BamHI
BclI
BglII
BssHII
DraI
EcoRI
EcoRV
HindIII
HinfI
HpaI
HpaII
KpnI
MluI
MspI
NarI
NcoI
NotI
NruI
PalI
PstI
PvuI
SacII
SalI
Sau3AI
ScaI
SmaI
SnaBI
SpeI
SrfI
TaqI
XbaI
Acetobacter aceti
Arthrobacter luteus
Acetobacter pasteurianus
Bacillus amyloliquefaciens
Bacillus caldolyticus
Bacillus globigii
Bacillus stearothermophilus
Deinococcus radiophilus
Escherichia coli
Escherichia coli
Haemophilus influenzae
Haemophilus influenzae
Haemophilus parainfluenzae
Haemophilus parainfluenzae
Klebsiella pneumoniae
Micrococcus luteus
Moraxella sp
Nocardia argentiensis
Nocardia corallina
Nocardia otitidis
Nocardia rubra
Providencia alcalifaciens
Providencia stuartii
Proteus vulgaris
Streptomyces achromogenes
Streptomyces albus
Staphylococcus aureus
Streptomyces caespitosus
Serratia marcescens
Sphaerotilus natans
Sphaerotilus sp
Streptomyces sp
Thermus aquaticus
Xanthomonas campestris
var badrii
Xanthomonas campestris
var holcicola
GACGT/C
AG/CT
GGGCC/C
G/GATCC
T/GATCA
A/GATCT
G/CGCGC
TTT/AAA
G/AATTC
GAT/ATC
A/AGCTT
G/ANTC
GTT/AACb
C/CGG
GGTAC/C
A/CGCGT
C/CGG
GG/CGCC
C/CATGG
GC/GGCCGCc
TCG/CGA
GG/CC
CTGCA/G
CGAT/CG
CCGC/GG
G/TCGAC
/GATC
AGT/ACT
CCC/GCCb
TAC/GTA
A/CTAGT
GCCC/GGGCc
T/CGA
Bacillus sphaericus
/(10/15) AC(4N)GTAYC(12/7)/
XhoI
BaeI
a
b
c
d
T/CTAGA
C/TCGAG
5 -to-3
restriction point
(REs); the REs cannot cleave DNA
in which these sites have been modified in one or both strands.
Modification does not interfere with normal base-pairing, so
that semiconservative replication of fully modified dsDNA will
result in two duplexes, each containing one (modified) parent
strand and one unmodified daughter strand. The modified parent
strand protects the duplex from restriction, and the daughter
strand is modified before further DNA replication; thus, DNA
susceptible to restriction does not normally occur in the cell.
However, if foreign DNA lacking the modification pattern of
the strain enters the cell (e.g. by conjugation, transformation,
phage infection etc) it will generally be degraded. (See also
HOST-CONTROLLED MODIFICATION.)
Certain bacteriophages encode their own RM systems: see
e.g. T-EVEN PHAGES and BACTERIOPHAGE MU.
restriction point (in cell cycle) See CELL CYCLE.
restrictive conditions See CONDITIONAL LETHAL MUTANT.
resupinate (mycol.) Refers to a fruiting body which forms a crust
on the surface of the substratum, the spore-bearing surface being
outermost.
reticle See MICROMETER.
reticulate body See CHLAMYDIA.
reticule See MICROMETER.
reticuloendotheliosis viruses See AVIAN RETICULOENDOTHELIOSIS
VIRUSES.
reticulopodium See PSEUDOPODIUM.
reticulum See RUMEN.
retinaculum apertum See SPIRA.
retinal The purple component of various photosensitive proteins, e.g. BACTERIORHODOPSIN, HALORHODOPSIN, SLOW-CYCLING
RHODOPSIN. The free retinal molecule is R[CH=CHC(CH3 )=
CH]2 CHO where R = 2,6,6-trimethyl-1-cyclohexenyl. (The
corresponding alcohol, retinol, is vitamin A.) Linkage of the
aldehyde group of retinal to a lysine residue in a halobacterial
opsin creates a Schiff base. The synthesis of retinal in Halobacterium salinarium is inhibited e.g. when the organism is grown
in the presence of nicotine.
retort (in canning) See BATCH RETORT.
retort pouch A flexible container used in the food processing industry as an alternative to the can. Typically, the pouch
is made of a laminate consisting of aluminium foil sandwiched between an outer layer of polyester and an inner layer
of e.g. polypropylene and nylon the layers being bonded
together by e.g. a polyesterisocyanate adhesive. (See also CANNING.)
Retortamonadida An order of parasitic protozoa (class
ZOOMASTIGOPHOREA). The cells, which are not bilaterally
symmetrical, have two to four flagella, one of which is directed
posteriorly along the ventral surface; cells lack mitochondria,
Golgi apparatus, an axostyle and an undulating membrane.
Genera: e.g. CHILOMASTIX, Retortamonas.
Retortamonas See RETORTAMONADIDA.
retrogressive development See CONIDIUM.
retrohoming See INTRON HOMING.
retroid viruses Viruses which resemble members of the RETROVIRIDAE in that they appear to employ a replication mechanism
which involves reverse transcription of an RNA intermediate;
retroid viruses include CAULIFLOWER MOSAIC VIRUS [review: TIBS
(1985) 10 205209] and members of the HEPADNAVIRIDAE. [Possible common evolutionary origin of hepatitis B virus and retroviruses: PNAS (1986) 83 25312535.]
RESTRICTION ENDONUCLEASES
656
Retroviridae
5 end
R
3 end
U5 ()PBS L
gag
pol
Cap
env
P
U3
[ (+)PBS?]
R
An
RETROVIRIDAE: Figure 1. The retrovirus genome, showing generalized features (not to scale). The genomes of some retroviruses have
additional coding sequences not shown here.
R
U5
() PBS
L
gag
pol
env
P
U3
Cap
An
=
=
=
=
=
=
=
=
=
=
=
Terminal redundancy.
Sequence unique to the 5 end (present at each end in proviral DNA).
Primer binding site for the () DNA strand primer (a host tRNA).
Leader sequence.
Group-specific antigen genes (coding region for nucleocapsid proteins).
Coding region for e.g. reverse transcriptase.
Coding region for envelope glycoprotein.
Polypurine tract and probable primer binding site for (+) DNA strand synthesis.
Sequence unique to the 3 end (present at each end in proviral DNA).
5 Cap nucleotide (m7 G5 ppp5 . . .), added after transcription and not copied during DNA synthesis.
3 Polyadenylate tract (e.g. ca. 100200 nucleotides long), added after transcription and not copied during DNA synthesis.
3
U3
R U5
RNA
3 5 R U5
R U5
U3
U3
R U5
R U5
R
U3
3 R U5
P U
U5
U3 R U5
U3 R U5
U3
R U5
U3 R U5
U3 R U5
U3 R U5
LTR
U3 R U5
LTR
RETROVIRIDAE: Figure 2. Model for retroviral dsDNA synthesis from the ssRNA genome. (Thin lines = RNA; thick lines = DNA.) (Continued
on page 659.)
658
reverse gyrase
all v-onc+ viruses are replication-defective: certain strains of
ROUS SARCOMA VIRUS contain the oncogene v-src in addition to a
full complement of viral genes.) All known v-onc+ viruses can
transform at least some type(s) of cell in culture; by contrast,
very few v-onc viruses can transform cells in culture (cf. HTLV),
although a few can cause CPE (e.g. vacuolization, syncytium
formation, cell death) usually only in certain types of cell.
(See also e.g. AVIAN LEUKOSIS VIRUSES, FELINE LEUKAEMIA VIRUS,
MURINE LEUKAEMIA VIRUSES; cf. FRIEND VIRUS and MCF VIRUSES.)
retroviruses Viruses of the RETROVIRIDAE.
retting The process by which cellulose fibres are released from
the stems of flax (Linum usitatissimum), hemp (Cannabis
sativa), or jute (Corchorus spp, Tiliaceae) by the action of
pectinolytic fungi and bacteria; these organisms soften the stems,
and the fibres are then separated by beating (scutching). The
fibres are used in the textile industry e.g. for the manufacture of
linen (from flax), hessian (from hemp or jute), twine (from hemp)
etc. In aerobic retting processes (dew retting) the organisms
involved include e.g. Cladosporium herbarum, Aureobasidium
pullulans, and species of Cryptococcus, Rhizopus, Rhodotorula,
Bacillus and Pseudomonas. In anaerobic processes the stems
are submerged in water-tanks, and the main retting agents are
Clostridium spp, especially C. felsineum.
REV (REV-T, REV-A) See AVIAN RETICULOENDOTHELIOSIS VIRUSES.
reversal reaction See LEPROSY.
reverse CAMP test See CAMP TEST.
reverse electron transport Energy-dependent (uphill) electron
flow along an ELECTRON TRANSPORT CHAIN (or part of an ETC);
the energy for reverse electron transport is derived from proton
motive force (see CHEMIOSMOSIS), and, in e.g. animal mitochondria, the electrons may derive from the oxidation of succinate.
Reverse electron transport is an essential process in e.g. photosynthetic bacteria of the Rhodospirillineae; in these organisms,
pmf derived from PHOTOSYNTHESIS is used not only for the synthesis of ATP but also for the generation of reducing equivalents
by uphill electron flow to NAD+ . In Thiobacillus ferrooxidans,
reduction of pyridine nucleotides is reported to involve uphill
electron flow through the bc1 /NADH-Q oxidoreductase complex acting in reverse [JB (2000) 182 36023606].
reverse gyrase A TOPOISOMERASE which can introduce positive
supercoiling into cccDNA, using the energy of ATP hydrolysis;
the enzyme has been found e.g. in the archaean Sulfolobus
acidocaldarius [Nature (1984) 309 669681] and in bacteria
of the order Thermotogales [JB (1991) 173 39213923] all
being thermophilic organisms. The function of reverse gyrase is
unknown, but one suggestion is that it may have an important
659
reverse mutation
both phases (reverse transcription and PCR proper) may be
carried out in a single tube [e.g. JCM (1999) 37 524530].
Reverse transcription, which requires a primer, is carried out
isothermally at e.g. 50 C. Such relatively low temperatures can
be problematic if the target RNA contains secondary structures
that are destabilized only at a higher temperature: the presence of
secondary structures can block the synthesis of cDNA by physically impeding the polymerase. The problem of secondary structures may be overcome by carrying out reverse transcription at a
higher temperature. This approach requires a thermostable polymerase such as the rTth DNA polymerase (Perkin-Elmer) a
recombinant form of the Thermus thermophilus enzyme which
can operate as a reverse transcriptase at 6070 C in the presence of Mn2+ and can also amplify DNA in the cycling phase
of PCR in the presence of Mg2+ .
rtPCR can be used e.g. to detect specific types of mRNA
molecule. It is particularly useful for studying RNA viruses;
examples include: dengue virus [JCM (1999) 37 25432547];
hepatitis G virus [JCM (1997) 35 767768]; hepatitis C virus
and HIV-1 [Lancet (1999) 353 359363].
reverse transcription See REVERSE TRANSCRIPTASE.
reversion Restoration of the original phenotype of a mutant
organism by means of a BACK MUTATION or a SUPPRESSOR
MUTATION; the resulting organism is called a revertant.
revertant See REVERSION.
Reyes syndrome An acute disease of children and adolescents; it
involves e.g. non-inflammatory encephalopathy with fatty infiltration and dysfunction of the liver, and is characterized clinically by persistent and profuse vomiting and neurological dysfunction sometimes progressing to delirium, coma and death.
The aetiology is unknown. The syndrome characteristically follows infection with certain viruses, particularly influenza A or
B or varicella-zoster viruses. An association has also been recognized between the occurrence of Reyes syndrome and the
administration of aspirin during the prodromal phase of the viral
infection; in the USA, decreasing use of salicylates in children
has apparently correlated with a decrease in the incidence of
Reyes syndrome [Pediatrics (1986) 77 598602].
RF Replicative form, an intermediate formed during the replication of certain ssDNA or ssRNA viral genomes; an RF is
a double-stranded structure consisting of the viral strand basepaired with its (newly synthesized) complementary strand. (cf.
RI.) In e.g. SSDNA PHAGES the RF is a circular dsDNA molecule;
the supercoiled ccc form is designated RFI (cf. DNA I), while the
relaxed form nicked in one strand is designated RFII (cf.
DNA II).
RF-1, RF-2, RF-3 See PROTEIN SYNTHESIS (termination).
rfb gene See EHEC.
RFLP Restriction fragment length polymorphism: a phrase
which refers to differences in fragment length which may be
obtained when related sequences of DNA are exposed to the
same RESTRICTION ENDONUCLEASE(S); such differences may arise
e.g. if sequence(s) have lost or gained one or more (relevant)
restriction sites as a result of mutation, or if particular fragment(s) are longer or shorter, respectively, as a result of insertion
or deletion of nucleotides. The concept of RFLP is illustrated in
the figure.
RFLP analysis is used e.g. for TYPING. For typing short
sequences (e.g. a plasmid, viral DNA, or a short sequence in
a bacterial chromosome), the fragments formed by restriction
are examined by electrophoresis and staining (thus providing
a fingerprint). This approach has been used e.g. for detecting
variation in the genome of herpes simplex virus type 1 [RMM
(1998) 9 217224].
Rhabdoviridae
1
rhabdovirus
members of the plant rhabdoviruses include e.g. carrot latent
virus, lucerne enation virus, raspberry vein chlorosis virus, and
strawberry crinkle virus (all aphid-borne); barley yellow striate
mosaic virus (= cereal striate virus), cereal chlorotic mottle
virus, finger millet mosaic virus, maize mosaic virus, oat striate
virus, rice transitory yellowing virus, Russian winter wheat
mosaic virus, and wheat chlorotic streak virus (all hopper-borne);
beet leaf curl virus (lace bug-borne); coffee ringspot virus
(mite-borne). Listed by the ICTV [Book ref. 23, pp. 112114]
as possible members are some non-enveloped viruses (e.g.
Citrus leprosis virus and orchid fleck virus) and many virus-like
particles; these appear to resemble rhabdovirus nucleocapsids
(ca. 100120 35 nm) and form characteristic spoked-wheel
structures in the plant cell nucleus.
rhabdovirus A virus of the RHABDOVIRIDAE.
rhamnogalacturonan See PECTINS.
rhamnolipid (2-O-a-L-rhamnopyranosyl-a-L-rhamnopyranosyl-bhydroxydecanoyl-b-hydroxydecanoate) An extracellular glycolipid BIOSURFACTANT produced by certain strains of Pseudomonas aeruginosa during growth on HYDROCARBONS.
L-rhamnose 6-Deoxy-L-mannose; it occurs e.g. in many plant
glycosides and PECTINS, many streptococcal C SUBSTANCES, and
some LIPOPOLYSACCHARIDES (e.g. the O-specific chains of certain
Salmonella serotypes).
Rhaphidophyceae See CHLOROMONADS.
rhapidosomes Rod-shaped or tubular structures, 2030 nm in
diameter, which occur in many species of bacteria (e.g. Flexibacter, Pseudomonas spp) and cyanobacteria (e.g. Spirulina).
Rhapidosomes (in different organisms) have been variously
regarded as bacteriocins, defective phage tails, particles of
mesosomal membrane, and cell components involved in motility.
Rheinberg illumination (coloured field illumination; optical staining) Illumination analogous to that used in low-power darkfield MICROSCOPY (q.v.). Instead of an opaque stop, the condenser
is fitted with a Rheinberg disc: a transparent disc with a central
circular area of one colour and a surrounding annulus of one
or more lighter colours; the central colour forms the background
light while the specimen is lit by the peripheral rays of the lighter
colour(s).
rheotaxis A TAXIS in which the stimulus is a current; a positively
rheotactic organism swims against a prevailing current (i.e., it
swims upstream).
rheotropism See TROPISM (sense 1).
rheumatic fever A condition which occurs as a late complication of SCARLET FEVER or a group A streptococcal infection
of the throat (strep throat, tonsillitis) or middle ear (OTITIS
MEDIA); it may follow an asymptomatic streptococcal infection, but rarely or never occurs after streptococcal skin infection
(e.g. IMPETIGO, ERYSIPELAS) cf. POST-STREPTOCOCCAL GLOMERULONEPHRITIS. Rheumatic fever occurs most commonly in children
aged between 5 and 15. An asymptomatic latent period of 13
weeks may occur between the original infection and the onset of
rheumatic fever. Onset is usually rather insidious, with malaise,
fever, and inflammation of joints; other symptoms may include
e.g. subcutaneous nodules, rash, and/or involuntary twitching
movements (Sydenhams chorea, St Vituss dance). Endocarditis may develop and may lead to chronic rheumatic valvular heart
disease. An individual who has suffered an attack of rheumatic
fever has greatly increased susceptibility to subsequent streptococcal infection. Rheumatic fever is apparently unrelated to the
presence of living streptococci and is believed to be caused by
an immunopathological mechanism; it may be due to an autoimmune reaction between anti-group A streptococcal antibody and
a host tissue component.
Rhizosolenia
rhizogenic Capable of inducing root formation.
rhizoid A root-like structure which forms part of the thallus
in certain algae and fungi; it may anchor the organism to the
substratum and/or act as an absorptive organ or organelle. (cf.
RHIZOMYCELIUM.)
rhizomania See BEET NECROTIC YELLOW VEIN VIRUS.
rhizomorph (mycol.) A macroscopic, typically dark-coloured
thread of hard, compacted tissue formed by certain higher fungi,
e.g. Armillaria mellea; the tissue generally appears to consist of
individual cells rather than hyphae. Rhizomorphs are enduring
structures which can remain dormant under adverse conditions
and which can enable a fungus to spread into the surrounding
environment e.g. those of A. mellea permit the fungus to
spread from an infected tree to an uninfected tree via the soil.
(See also DRY ROT.)
Rhizomucor A genus of fungi of the MUCORALES. R. pusillus
(formerly Mucor pusillus) can cause ZYGOMYCOSIS. (See also
COMPOSTING.) R. miehei (formerly Mucor miehei ) and R. pusillus
form PROTEASES which are used as rennin substitutes.
rhizomycelium (mycol.) Branching, anucleate or sparsely nucleate, rhizoidal filaments of variable width which form part of
the thallus e.g. of Nowakowskiella and of some species of the
Laboulbeniales.
Rhizophidium See RHIZOPHYDIUM.
Rhizophydium (Rhizophidium) A genus of eucarpic fungi (order
CHYTRIDIALES) which occur as saprotrophs or as parasites of
aquatic or terrestrial plants; R. graminis parasitizes the root cells
of mono- and dicotyledonous plants (apparently without causing
them harm), while R. couchii has been reported to parasitize
Spirogyra. In the asexual cycle of R. couchii, a zoospore encysts
on the surface of a host and gives rise to a thallus whose
rhizoids penetrate the host; the extracellular part of the thallus
subsequently becomes converted into a zoosporangium. In the
sexual cycle, zoospores develop into extracellular, rhizoidbearing gametangia; after plasmogamy (and karyogamy?) the
zygote becomes a thick-walled resting zoosporangium.
rhizoplane The root surface cf. RHIZOSPHERE.
rhizoplasmodium See LABYRINTHULAS.
rhizopod An organism of the RHIZOPODA.
Rhizopoda A superclass of protozoa (subphylum SARCODINA)
which are motile by means of lobopodia, filopodia or reticulopodia (see PSEUDOPODIUM) or by flow of protoplasm without
the formation of discrete pseudopodia. Classes: ACARPOMYXEA;
Acrasea (see ACRASIOMYCETES); EUMYCETOZOEA; FILOSEA; GRANULORETICULOSEA; LOBOSEA; Plasmodiophorea (= PLASMODIOPHOROMYCETES); XENOPHYOPHOREA.
rhizopodium See PSEUDOPODIUM.
Rhizopogon See GASTEROMYCETES (Hymenogastrales).
Rhizopus
A genus of fungi (order MUCORALES) which occur
on soil, fruit etc. The organisms form a branched, aseptate
mycelium. R. nigricans (= R. stolonifer) can attach to the substratum by means of branching rhizoids; a stolon (a surface
hypha analogous to the stolons in higher plants) grows for some
distance and then gives rise to more rhizoids and to one or more
vertical sporangiophores. The organisms form ZYGOSPORES (see
also COMPATIBILITY sense 2). Rhizopus spp are used commercially e.g. in the preparation of ONCOM, RAGI and TEMPEH and in
certain STEROID BIOCONVERSIONS. (See also BREAD SPOILAGE and
ZYGOMYCOSIS.)
Rhizosolenia A genus of freshwater and marine centric DIATOMS.
Some (marine) species contain a nitrogen-fixing cyanobacterial symbiont, Richelia intracellularis, which occurs as short,
Calothrix-like filaments each with a heterocyst at one end or,
rhizosphere
in the dividing diatom, at both ends. The association is not
obligatory, and Richelia may also be found free-living or as
an epiphyte on diatoms of the genera Chaetoceros, Hemiaulus
and Rhizosolenia. (cf. RHOPALODIA.)
rhizosphere An environment regarded, variously, as e.g. (a) that
region of the soil which is modified as a result of the uptake
and deposition of substances by a growing root [AEE (1985)
12 99116]; (b) the root itself, together with that volume of
soil which it influences [Book ref. 112, p. 237]; or (c) the
root surface (rhizoplane) together with that region of the
surrounding soil in which the microbial population is affected,
qualitatively and/or quantitatively, by the presence of a root. The
rhizosphere may extend a few millimetres, or centimetres, from
the rhizoplane.
From a growing root, a number of substances pass out into the
soil. These substances include various carbohydrates (see also
MUCIGEL), vitamins, amino acids and sugars many of which
serve as nutrients and/or as sources of energy for microorganisms. Presumably as a result of this, the microflora of the
rhizosphere differs appreciably from that of the surrounding soil.
In the rhizosphere, bacterial numbers are often 10- to 50-fold
higher than they are in the surrounding soil; the bacteria are
mainly Gram-negative rods (e.g. pseudomonads), Gram-positive
bacteria typically being less numerous than they are outside
the rhizosphere. It has been reported that the presence of a
vesicular-arbuscular MYCORRHIZA (involving Glomus fasciculatum) reduces the proportion of fluorescent pseudomonads and
increases the proportion of facultatively anaerobic bacteria in
the rhizosphere but does not affect the absolute number of
Gram-negative bacteria [SBB (1986) 18 191196].
Numerically, fungi may be present in similar or slightly
greater abundance in the rhizosphere as compared with the
surrounding soil. However, there may be qualitative (species)
differences between rhizosphere and non-rhizosphere fungi, and
in at least some cases there is evidence that the rhizospheres of
certain plants encourage, or select, particular fungi.
The extent to which the plant benefits from the rhizosphere
microflora remains unclear. It seems possible that the microflora
may play some part in protecting the plant from the incursions
of soil-borne pathogens; additionally, the plant may benefit from
the mineralizing activities of these organisms, and it is generally
believed that the presence of the rhizosphere microflora promotes
the uptake of minerals (e.g. phosphate) by the root.
rhizothamnium A Myrica-type ACTINORRHIZA.
rhl genes See QUORUM SENSING.
rho factor (r factor) See TRANSCRIPTION.
rho-form See MYCOPLASMA (M. mycoides).
rho gene In e.g. Escherichia coli : the gene encoding the r factor
(see TRANSCRIPTION).
rho petite See PETITE MUTANT.
rho0 petite See PETITE MUTANT.
rhodamine A generic term for a group of substituted xanthene FLUOROCHROME dyes; examples: rhodamine B (fluorescence red see also AURAMINERHODAMINE STAIN and LISSAMINE
RHODAMINE), rhodamine S (fluorescence yellow), rhodamine O
(red), rhodamine 3G (orange). The rhodamines include cationic,
anionic and neutral dyes. Uptake of cationic rhodamines (e.g.
rhodamine 123) appears to depend on membrane potential in
viable, functioning mitochondria [JCB (1981) 88 526535] and
bacteria [FEMS (1984) 21 153157]. (See also VITAL STAINING.)
rhodanese (thiosulphate sulphurtransferase; EC 2.8.1.1) An enzyme that catalyses e.g. the formation of thiocyanate (SCN )
and sulphite (SO3 2 ) from THIOSULPHATE and cyanide; it
Rhodospirillaceae
prosthecae. (Branches arise from the filaments.) Each cell is
separated from its neighbour by a plug formed within the filament joining them. Such arrays apparently the commonest
form under natural conditions may be produced under conditions of high light intensity and low concentrations of CO2 . If the
light dims and CO2 levels rise (e.g. as the array becomes large),
motile (peritrichous) swarmer cells form at the ends of filaments
and are released by binary fission; under suitable conditions
swarmers shed their flagella and become non-motile prosthecate cells, thus completing the cycle. If conditions of low light
and high CO2 persist, a second (simplified) cell cycle occurs:
arrays are not formed budding cells giving rise only to swarmers; array formation can subsequently occur if CO2 concentration
decreases and light intensity increases. Under starvation conditions, cell arrays give rise to exospores: angular structures,
resistant to heat and drying, which form at the tips of filaments
and are released by binary fission; the exospores can germinate
under aerobic conditions in the dark or anaerobically in the light,
forming up to four vegetative cells. (Exospores are not formed
in the simplified cycle; late exponential phase cultures contain
tiny cells which are not resistant to stress [JGM (1980) 117
4755].)
[Reviews: ARM (1981) 35 567594; Book ref. 28, pp. 188
210.]
(See also HYPHOMICROBIUM.)
rhodomycin See ANTHRACYCLINE ANTIBIOTICS.
Rhodophyceae See RHODOPHYTA.
Rhodophyta (red algae) A division of ALGAE. Over 95% of
the ca. 5000 species of red algae are marine organisms;
those which occur in freshwater and/or soil habitats include
species of Audouinella, Bangia, Batrachospermum, Chroodactylon, Hildenbrandia, Lemanea and Porphyridium. (Some genera,
e.g. Bangia, Bostrychia and Hildenbrandia, contain both marine
species and freshwater species.) A few red algae are parasitic on
other algae (see e.g. CHOREOCOLAX and HOLMSELLA).
In most red algae the thallus is a branched filament or
ribbon. However, some species are sheet-like (e.g. Porphyra) or
crust-like (e.g. Lithophyllum), while a few (e.g. PORPHYRIDIUM)
are unicellular. Some red algae are calcified e.g. Corallina
spp (thalli: erect, articulated) and Lithophyllum. Multicellular
thalli (which are commonly 550 cm in length) are typically
attached to rocks etc by a holdfast. The CELL WALL may contain
cellulose or xylans. Plasmodesmata appear to be absent, but
many multicellular red algae contain PIT CONNECTIONS. There are
no flagellated species, and flagellated gametes are not produced.
Marine species are usually some shade of red, while freshwater
species are typically blue-green, yellow-green, brown or grey.
Red algae contain CHLOROPHYLL a, and some also contain chlorophyll d ; the THYLAKOIDS occur singly (i.e., unassociated) and bear PHYCOBILISOMES containing phycoerythrins
and/or phycocyanins. Various CAROTENOIDS (e.g. xanthophylls
and b-carotene) are usually present. Storage products include
FLORIDEAN STARCH and FLORIDOSIDE (see also ISOFLORIDOSIDE).
Sexual reproduction occurs in most species (but apparently
not in Porphyridium) and oogamy is common; life cycles are
often complex.
Certain red algae are used as sources of AGAR and CARRAGEENAN, while some are used as food (see e.g. LAVER, NUNGHAM, PALMARIA).
All species are placed in one class: Rhodophyceae.
Orders [Book ref. 130]: Bangiales (e.g. Bangia, PORPHYRA);
Ceramiales (e.g. Bostrychia; Ceramium, Griffithsia, Polysiphonia); Compsopogonales (e.g. Compsopogon); Cryptonemiales (e.g. CHOREOCOLAX, Corallina, Gloiopeltis, Hildenbrandia, HOLMSELLA, Lithophyllum); Gigartinales (e.g. Chondrococcus, Chondrus, Eucheuma, Furcellaria, Gardneriella, GIGARTINA,
Gracilaria, Iridaea); Nemalionales (e.g. Audouinella, Batrachospermum, Gelidium, Lemanea); Palmariales (e.g. Palmaria);
Porphyridiales (e.g. Chroodactylon, Cyanidium, PORPHYRIDIUM);
Rhodochaetales (e.g. Rhodochaete); Rhodymeniales (e.g. Coeloseira, Rhodymenia).
[Biology of freshwater red algae: Book ref. 167, pp. 89157.]
Rhodopila
A proposed genus of bacteria [IJSB (1984) 34
340343] which includes a species transferred from RHODOPSEUDOMONAS (q.v.) and re-designated Rhodopila globiformis; the
coccoid, flagellated cells of R. globiformis grow only at low
pH.
Rhodopseudomonas A genus of photosynthetic bacteria (family RHODOSPIRILLACEAE). Cells: flagellated (or non-motile) rods
or cocci, typically 15 m; most species contain Bchl a,
R. sulfoviridis and R. viridis contain Bchl b. R. acidophila,
R. palustris (the type species), R. sulfoviridis and R. viridis
divide by budding; other species divide by binary fission.
R. palustris and R. viridis form prosthecae. The oval to rodshaped species R. adriatica, R. capsulata, R. sphaeroides and
R. sulfidophila all have vesicular-type photosynthetic membranes, and it has been proposed that they be transferred to a new
genus: RHODOBACTER; it has also been proposed that the coccoid
species R. globiformis (which has a vesicular photosynthetic
membrane) and the curved, rod-shaped species R. gelatinosa be
transferred to the genera RHODOPILA and RHODOCYCLUS, respectively [IJSB (1984) 34 340343].
[Gene transfer mechanisms: Ann. Mic. (1983) 134 B 195
204.] (See also CAPSDUCTION.)
Rhodospirillaceae (purple non-sulphur bacteria, or non-sulphur
purple bacteria; Athiorhodaceae) A heterogeneous family
(see RHODOSPIRILLALES) of photosynthetic bacteria (suborder
RHODOSPIRILLINEAE); they occur typically in those anaerobic
habitats in which a range of simple organic substrates
has been made available by the metabolic activities of
chemoorganotrophic bacteria e.g. in the mud of ponds and
rivers, and in sewage lagoons. The organisms occur in
freshwater, brackish and marine habitats and in moist soils. Most
species contain only Bchl a (two species of Rhodopseudomonas
have only Bchl b) see CHLOROPHYLLS; these pigments, and
various carotenoids, occur in lamellar, tubular or vesicular
intracytoplasmic membrane systems, according to species.
The organisms include cocci, rods and spiral forms; most
species divide by binary fission, but several divide by
budding (see e.g. RHODOPSEUDOMONAS). Heat-resistant forms are
produced by Rhodomicrobium vannielii. Most species (not e.g.
Rhodocyclus purpureus) exhibit flagellar motility. Gas vacuoles
are absent. The organisms are primarily photoorganotrophic
heterotrophs under anaerobic conditions, but a few species, e.g.
Rhodopseudomonas sulfidophila, can grow as photolithotrophic
autotrophs (using sulphide as electron donor), and some other
members of the family can use sulphide as electron donor
only when it is present in low concentrations. It has been
shown that at least some species can oxidize elemental sulphur
[JGM (1985) 131 791798]; sulphide (or thiosulphate) can
be oxidized to sulphate (without sulphur formation) by e.g.
Rhodopseudomonas sulfidophila. Many species can oxidize
sulphide with the production of extracellular deposits of sulphur.
A number of species can use hydrogen as an electron donor for
665
Rhodospirillales
plant debris, beverages, pickling brines (see also SAUERKRAUT),
seawater, fresh water, etc. [Book ref. 100, pp. 893905.]
Rhodymenia See RHODOPHYTA (cf. PALMARIA).
Rhopalodia A genus of pennate DIATOMS. The freshwater species
R. gibba and R. gibberula contain, in addition to the typical
diatom chloroplast, intracellular inclusion bodies which closely
resemble thin-walled unicellular cyanobacteria and which carry
out light-dependent nitrogen fixation. (cf. RHIZOSOLENIA.)
Rhopalomyces See ZOOPAGALES.
rhoptries (sing. rhoptry) In members of the APICOMPLEXA: elongate (e.g. club-shaped) osmiophilic organelles found at the anterior end of the cell; two such organelles per cell occur e.g. in
the merozoites of Isospora spp and many Eimeria spp, while
more than two per cell occur e.g. in some Eimeria merozoites
and in Sarcocystis and Toxoplasma. Rhoptries appear to secrete
enzymes which assist in host cell penetration [JUR (1983) 83
8598].
RHP (Rhodospirillum haem protein; cytochromoid c) Original
name for CYTOCHROMES c and cc which occur in at least some
purple phototrophic bacteria and in Pseudomonas denitrificans.
Rhynchodida See HYPOSTOMATIA.
Rhynchoidomonas
A genus of monoxenous protozoa (family TRYPANOSOMATIDAE) parasitic in the gut (particularly the
Malpighian tubules) of flies. The organisms, 1050 m long,
occur in the trypomastigote form but lack a free flagellum.
Rhynchomonas See BODONINA.
rhynchosporium A plant disease caused by Rhynchosporium sp:
see e.g. LEAF BLOTCH.
Rhynchosporium See HYPHOMYCETES; see also LEAF BLOTCH.
Rhytidhysteron See ASCOSTROMA.
Rhytisma A genus of fungi of the RHYTISMATALES. R. acerinum
causes tar spot disease in Acer spp (e.g. maple): conspicuous,
flat, roundish, black stromata (ca. 12 cm diam.) develop on
the upper surfaces of leaves from mid-summer onwards, the
stromata bearing conidiophores of the imperfect (Melasmia)
stage during the autumn; ascocarps (the over-wintering stage)
develop within the stromata, each stroma splitting radially in
the spring to expose the apothecial hymenia of asci containing
filiform ascospores.
Rhytismatales An order of fungi (subdivision ASCOMYCOTINA)
which include saprotrophic and plant-parasitic species. Ascocarp: APOTHECIOID, immersed in a stroma or in host tissue;
hamathecium: filiform paraphyses. Asci: unitunicate; sometimes
stipitate. Ascospores: septate or aseptate. Genera: e.g. Coccomyces, Hypoderma, RHYTISMA.
RI Replicative intermediate, an intermediate formed during the
replication of certain ssRNA viral genomes; an RI is a partially
double-stranded structure with many (growing) single-stranded
tails formed as a result of the concomitant synthesis of many
new RNA strands on the same RNA template strand. (cf. RF.)
Ri plasmid See HAIRY ROOT.
RIA RADIOIMMUNOASSAY.
RIBA See HEPATITIS C.
ribavirin (1-b-D-ribofuranosyl-1,2,4-triazole-3-carboxamide; Virazole) An ANTIVIRAL AGENT which is active against a wide range
of viruses and which has been used therapeutically against infections caused e.g. by the hepatitis C, Lassa fever and SARS
(coronavirus) viruses.
Ribavirin is phosphorylated in cells; the monophosphate
inhibits IMP dehydrogenase (and hence GMP and GTP synthesis: see Appendix V(a)), while the triphosphate directly inhibits
e.g. influenzavirus RNA-dependent RNA polymerase. A suggestion that ribavirin may act as a cap analogue (see MRNA (b)) was
not confirmed [RNA (2005) 11 12381244].
ribosome
RiboPrinter An automated system (manufactured by Qualicon,
Wilmington, DE, USA) designed for rapidly characterizing a
bacterium to strain level on the basis of its ribotype. The
apparatus is intended primarily for use in the food industry, and
its database contains ribotype patterns of hundreds of strains
of food-borne pathogens (with which the ribotypes of new
isolates can be compared). [Comparison of the RiboPrinter
with traditional ribotyping: LAM (1999) 28 327333.]
[Use of automated riboprinter and PFGE for epidemiological
studies of Haemophilus influenzae in Taiwan: JMM (2001) 50
277283.]
ribose An aldopentose (see PENTOSES) which plays many important roles in cell structure and metabolism. Phosphorylated
derivatives of ribose and 2-deoxyribose are components of
NUCLEOTIDES and NUCLEIC ACIDS [see also Appendix V(a) and
(b)], and ribose phosphates are important intermediates in certain metabolic pathways: e.g. CALVIN CYCLE, HEXOSE MONOPHOSPHATE PATHWAY [Appendix I(b)], biosynthesis of phenylalanine,
tyrosine and tryptophan [Appendix IV(f)] and of histidine
[Appendix IV(g)], etc. [See also Appendix III(d).]
ribose phosphate pathway Syn. RMP PATHWAY.
ribosome A ribonucleoprotein intracellular organelle (about
2530 nm in diameter) which mediates PROTEIN SYNTHESIS
(q.v. for function). Some ribosomes occur in the cytoplasm;
others (see e.g. ENDOPLASMIC RETICULUM) are membrane-bound.
Ribosomes are usually present in large numbers in the cell.
Each ribosome consists of two subunits one larger than the
other; both subunits contain RNA and protein.
Different types of ribosome are characterized by different
sedimentation coefficients (S) on ultracentrifugation (see also
SVEDBERG UNIT). Bacterial ribosomes have a sedimentation coefficient of ca. 70S; each consists of one 30S subunit and one
50S subunit. Ribosomes of the eukaryotic cell cytoplasm have
a sedimentation coefficient of ca. 80S; each consists of one 40S
subunit and one 60S subunit. Other ribosomes reported: those
in mammalian mitochondria (ca. 60S), in chloroplasts of plants
and algae (ca. 70S), in mitochondria of plants (ca. 78S), and
those in the mitochondria of yeasts and other lower eukaryotes
(ca. 73S).
CH2
N
O
H
OH OH OH
O
O
CH2
H3C
CH2
N9
N1
OH
OH
6
H3C
NH
N
5
10
3
4
O
adenosine 5-phosphate
riboflavin
flavin mononucleotide (FMN)
667
ribosome
resulting in the formation of HAIRPINS and STEM-AND-LOOP
etc. [rRNA structure: ARB (1984) 53 119162.]
The integrity of a ribosome appears to involve hydrogenbonding and both ionic and hydrophobic interactions, magnesium ions generally playing an important role in maintaining the
structure.
The basic architecture of a ribosome has been strongly conserved during evolution, although ribosomes from e.g. bacteria,
the eukaryotic cytoplasm and archaeans appear to show certain
distinctive morphological features (cf. PHOTOCYTA.) [Evolving ribosome structure: ARB (1985) 54 507530. Threedimensional model of the E. coli ribosome: Prog. Biophys. Mol.
Biol. (1986) 48 67101.]
Taxonomic role of rRNA. Certain regions of rRNA have been
very highly conserved during evolution, and sequence homology
studies in rRNAs are widely used to indicate evolutionary
relationships among organisms. [Evolutionary changes in 5S
rRNA higher order structure: NAR (1987) 15 161179.] (See
also RIBOTYPING.)
Biogenesis of ribosomes. Biogenesis appears to involve an
assembly process in which, initially, some of the r-proteins bind
to particular regions of rRNA; other r-proteins then bind cooperatively to this core structure. [ProteinrRNA recognition
and ribosome assembly: Book ref. 84, pp 331352.]
In rapidly growing cells of E. coli the number of ribosomes
per cell is essentially proportional to the growth rate; this
necessitates control mechanisms for co-ordinated expression of
the genes encoding r-proteins and rRNAs.
Genes encoding the r-proteins are grouped into a number
of distinct OPERONS. For example, the str operon contains
genes for (in order of transcription) S22, S7 and translation
elongation factors EF-G and EF-Tu (see PROTEINS SYNTHESIS);
the a operon contains genes for S13, S11, S4, RNA polymerase
subunit a and L17; the b operon contains genes for L10, L7/12
and RNA polymerase subunits b and b . Co-ordination of the
synthesis of r-proteins involves post-transcriptional AUTOGENOUS
REGULATION (translational feedback regulation). One model for
the control of these operons postulates that one of the r-proteins
encoded by a given operon acts as a regulatory molecule
(translational repressor) for that operon by binding to its own
(polycistronic) mRNA and blocking translation of some or all
of the encoded proteins; thus, for example, in the b operon L10
represses the translation of L10 and L7/L12, but not of the cotranscribed RNA polymerase b and b subunits. (See also RPO
GENES.) The E. coli IF3L35L20 operon contains the genes
infCrpmIrplT which encode (respectively) initiation factor
IF3 (see PROTEIN SYNTHESIS) and the r-proteins L35 (sic) and
L20; IF3 acts as a repressor of its own gene, and L20 apparently
acts as a translational repressor (in a concentration-dependent
way) by binding to a site (a translational operator ) upstream
of the rpmI sequence in the mRNA, thus blocking translation
of both r-proteins. The mechanism of repression by L20 is
unknown, but translational control of the operon apparently
involves a pseudoknot which affects the control region of rpmI
[EMBO (1996) 15 44024413].
Some of the operon-regulatory proteins also have binding sites
on either 16S or 23S rRNA. It is thought that, if the growth
rate decreases, the decreased amount of 16S and 23S rRNA
available in nascent ribosomes will leave these proteins free
to inhibit translation of their respective transcripts. Note that,
in this model, synthesis of ribosomal proteins is linked to the
availability of rRNA, regulation of the rRNA genes being the
key step in regulating the biogenesis of ribosomes; a ribosome
STRUCTURES
668
rice-straw mushroom
rickettsiae (1) Organisms of the RICKETTSIACEAE. (2) Organisms
of the genus RICKETTSIA.
Rickettsiales An order of Gram-negative bacteria which includes
the families ANAPLAMATACEAE and RICKETTSIACEAE.
rickettsialpox An acute, usually mild disease of man caused by
Rickettsia akari. House mice seem to be the main reservoir of
infection; the mite Allodermanyssus sanguineus transmits the
pathogen to man. Incubation period: 10 days to 3 weeks. There
may be a lesion at the site of the mite bite, and this is followed
by sudden onset of fever with headache, chills, anorexia and
photophobia; there may be a sparse maculopapular rash. The
disease is usually self-limiting; no deaths have been reported.
Rickettsieae A tribe of bacteria of the RICKETTSIACEAE comprising the genera COXIELLA and RICKETTSIA. The genus Rochalimaea
(including R. quintana, formerly Rickettsia quintana) has been
unified with the genus BARTONELLA (q.v.).
Rickettsiella A genus of Gram-negative bacteria of the tribe WOLBACHIEAE; species grow intracellularly in, and are pathogenic in,
arthropod hosts (including arachnids, crustaceans and insects).
Growth does not occur in cell-free media. Cells: rod- or discshaped, maximum dimension typically <0.8 m. The species:
R. chironomi (parasitic e.g. in midges and spiders); R. grylli
(e.g. in crickets Gryllus spp and the desert locust Schistocerca gregaria); R. popilliae (in various beetles including the
Japanese beetle, Popillia japonica and the crane fly).
rickettsiosis Any disease caused by a species of RICKETTSIA.
Rickia See LABOULBENIALES.
RidealWalker test A SUSPENSION TEST used to determine the
PHENOL COEFFICIENT of a (phenolic) disinfectant; the test determines that dilution of the test disinfectant which gives the
same rate of kill of a test organism as does a standard dilution of phenol. Serial dilutions (in water) of the test disinfectant
are equilibrated at 1718 C. Each dilution (5 ml) is inoculated
with a 24-hour broth culture (0.2 ml) of the test organism (e.g.
Salmonella typhi NCTC 786) and incubated at 1718 C. After
2.5, 5, 7.5 and 10 minutes, a standard loopful of the test suspension (from each dilution) is transferred to a separate volume of
sterile broth which is incubated at 37 C for 23 days to detect
surviving cells. A similar procedure is carried out with phenol.
For one particular dilution of the test disinfectant, growth will
occur in broths inoculated at 2.5 and 5 minutes but not in those
inoculated at 7.5 and 10 minutes; a similar result will be obtained
for one particular dilution of phenol (within the range 1/95 to
1/115 w/v). The phenol coefficient (RidealWalker coefficient )
is given by the ratio of the dilution factors of these two particular
dilutions:
dilution factor of test disinfectant
dilution factor of phenol
RIST
ring slide A slide used e.g. in some serological tests; it is larger
and thicker than a normal microscope SLIDE, and on one face it
has a number of fixed, raised rings (1 to 3 cm in diameter) made
of ceramic or other material.
ring spot See RINGSPOT.
ring stage (of Plasmodium) See PLASMODIUM.
ring test (serol.) A qualitative PRECIPITIN TEST, carried out in a
narrow tube, in which a solution containing antigen is layered
over one containing antibody. A positive reaction is indicated
by a band of white precipitate which forms at the interface of
the two solutions.
ring vaccination (vet.) Vaccination of animals in the annular
region surrounding an isolated outbreak of disease; the object
is to contain (i.e. prevent the spread of) the disease.
Ringers solution A solution used e.g. as a general diluent;
composition (g/100 ml distilled water): NaCl (0.9), KCl (0.042),
CaCl2 (0.048), NaHCO3 (0.02).
ringspot (plant pathol.) A type of LOCAL LESION consisting of
single or concentric rings of discoloration or necrosis, the regions
between the concentric rings being green; the centre of the lesion
may be chlorotic or necrotic.
ringworm (dermatophytosis; tinea) Any MYCOSIS of man and
animals in which keratinized tissues (skin, hair, nails etc) are
infected by a DERMATOPHYTE (q.v.). Infection occurs by direct
contact with an infected individual or with fomites. Ringworm infections in man may be categorized according to the
area of the body involved: tinea barbae = beard ringworm;
tinea capitis (tinea tonsurans) = scalp ringworm, caused e.g.
by Microsporum audouinii, M. canis or Trichophyton schoenleinii (cf. FAVUS); tinea corporis (tinea circinata) = body ringworm, caused e.g. by Microsporum or Trichophyton spp; tinea
cruris = groin ringworm, caused e.g. by Epidermophyton cruris;
tinea manus = hand ringworm; tinea pedis (ATHLETES FOOT) =
foot ringworm; tinea unguium = nail ringworm, caused e.g. by
T. mentagrophytes or T. rubrum. Lesions on skin are typically
circular or ring-shaped (sometimes coalescing to become confluent), dry and scaling (but cf. KERION), and may or may not
be painful or pruritic. Usually only the superficial layers of
skin are affected. Adults are generally less susceptible to skin
infection than are children owing to the fungistatic properties
of fatty acids in the sebum. Infected nails become opaque and
discoloured, distorted, and hard or flaky. Infected hairs usually
break. Lab. diagnosis: e.g. microscopic and cultural examination of epidermal scales and hairs. Under WOODS LAMP, hairs
infected with certain dermatophytes show characteristic fluorescence: e.g. hairs infected with M. audouinii or M. canis fluoresce bright green; those infected with Trichophyton spp may
appear a (non-diagnostic) bluish-white colour. Chemotherapy:
e.g. oral GRISEOFULVIN or POLYENE ANTIBIOTICS; topical ointments
containing e.g. tolnaftate or salicylic, benzoic or propionic acids.
Rio Bravo virus See FLAVIVIRIDAE.
Rio Grande virus See PHLEBOVIRUS.
RISE-resistant tuberculosis TUBERCULOSIS which is resistant
to treatment with a number of antibiotics, including at
least r ifampin, i soniazid, streptomycin and ethambutol.
[RISE-resistant tuberculous meningitis in an AIDS patient:
Lancet (1993) 341 177178.]
riser In a LOOP FERMENTER: the ascending column of liquid or
that part of the fermenter which contains it. (cf. DOWNCOMER.)
rishitin A sesquiterpenoid PHYTOALEXIN produced by potato
tubers.
RIST (radioimmunosorbent test) An IMMUNOASSAY used e.g. for
quantifying IgE in serum. Essentially, immobilized anti-IgE
medium. In aqueous oxygenated solutions rifamycin B spontaneously gives rise to e.g. rifamycins O and S which show much
higher antibacterial activity than rifamycin B itself. Rifamycin S
is an important starting point for the production of semisynthetic
rifamycins which include e.g. rifamycin SV (= rifamycin,
obtained by mild reduction of rifamycin S), rifamide, and
rifampicin (= rifampin).
Rifamycins are generally highly active against Gram-positive
bacteria (including mycobacteria, staphylococci and streptococci) and against some Gram-negative bacteria (e.g. Brucella, Chlamydia, Haemophilus, Legionella and Neisseria spp);
other Gram-negative bacteria (e.g. enterobacteria) are less sensitive, spirochaetes and mycoplasmas are insensitive. Rifamycins
specifically inhibit bacterial DNA-dependent RNA POLYMERASE,
binding to the b subunit and inhibiting initiation of transcription. Resistance to rifamycins may result from e.g. a mutation
which modifies the RNA polymerase b subunit such that it no
longer binds to the drug. Rifamycins do not inhibit mammalian
RNA polymerase or bacterial PRIMASE.
In some countries (including the USA), strains of Mycobacterium tuberculosis that are resistant to rifampicin are usually
also resistant to at least certain other anti-tuberculosis drugs, so
that resistance to rifampicin is a useful marker for multidrugresistant strains of the pathogen [see e.g. JAMA (1994) 271
665671].
Resistance-conferring mutations occur at a number of sites
in the rpoB gene (which encodes the b subunit of RNA
polymerase), and specific mutations may occur with different
frequencies in different geographical areas [e.g. Italy: JCM
(1999) 37 11971199].
Using DNA chip technology, high-density arrays have been
used to identify M. tuberculosis and, simultaneously, to test for
resistance to rifampicin [JCM (1999) 37 4955].
Rift Valley fever An acute, febrile disease of man and e.g. cattle,
sheep, camels, rats, mice etc; it occurs in Africa. The causal
agent, a virus of the genus PHLEBOVIRUS, is transmitted mainly
by insects (chiefly mosquitoes); rodents may provide a reservoir
of the virus. In lambs and calves, the incubation period is ca. 12
hours; onset is sudden, with high fever, hepatitis, incoordination,
collapse and (usually) death within 36 hours. In adult sheep and
cattle the main symptom is abortion, but there may be high fever
and a mortality rate of ca. 2030% in sheep, 10% in cattle. In
man, the disease resembles influenza; onset is abrupt, with chills,
fever, headache, myalgia and arthralgia. The disease is rarely
fatal in man, but retinal haemorrhages may lead to (temporary
or permanent) visual impairment.
Riftia See TROPHOSOME.
right-handed DNA See DNA.
right splice site See SPLIT GENE.
Rigidoporus See APHYLLOPHORALES (Polyporaceae).
Riley virus Syn. LACTATE DEHYDROGENASE VIRUS.
rimantadine See AMANTADINE.
rinderpest (bovine typhus; cattle plague) An acute, often fatal
CATTLE DISEASE which occurs e.g. in parts of Africa and Asia;
other animals, e.g. pigs, are also susceptible. The causal agent is
a Morbillivirus, and infection apparently occurs by inhalation of
aerosols. Incubation period (in cattle): ca. 1 week. Symptoms:
fever and anorexia, followed by lesions in the mouth and a
purulent nasal discharge; necrotic lesions appear on the lips and
gums, and severe diarrhoea follows the development of intestinal
lesions. Mortality rates may be very high. (cf. PESTE DES PETITS
RUMINANTS.)
ring-infected erythrocyte surface antigen See PLASMODIUM.
671
ristocetin
forms E4P and Xu5P; Xu5P is converted (by an epimerase)
to Ru5P, and E4P condenses with DHAP to form sedoheptulose
1,7-bisphosphate which is then converted (by sedoheptulose
bisphosphatase) to S7P. S7P with G3P forms ribose 5-phosphate
and Xu5P, each of which is converted (by an isomerase and an
epimerase, respectively) to Ru5P.
In some methylotrophic bacteria the RMP pathway can be
used to generate energy from certain substrates. This involves
a modified EntnerDoudoroff route in phase 2: a dehydrogenase (EC 1.1.1.44) converts 6-phosphogluconate to Ru5P with
concomitant elimination of CO2 and reduction of NAD(P).
In the assimilatory mode, the consumption of energy by
the RMP pathway varies according to the particular routes
taken in phases 2 and 3. Thus, e.g. a combination of the
EntnerDoudoroff route in phase 2 and the sedoheptulose
bisphosphate route in phase 3 consumes the largest amount of
energy; no organism has been reported to use this combination.
The (energetically) most economical routes of the RMP pathway
consume less energy than does either the SERINE PATHWAY or the
XMP PATHWAY.
Rms148, Rms149 plasmids See INCOMPATIBILITY.
RNA Ribonucleic acid: a NUCLEIC ACID consisting of riboNUCLEOTIDES, each of which contains one of the bases adenine,
guanine, cytosine or uracil, or, in some RNAs, a modified
form of one of these bases. (cf. DNA.) The 2 -OH group in
the RNA backbone makes the molecule more reactive and less
flexible than DNA. RNA molecules are usually single-stranded,
but an RNA strand can form a duplex (resembling A-DNA in
conformation) with a complementary strand of RNA or DNA;
ssRNA molecules commonly adopt secondary structures (e.g.
HAIRPINS, STEM-AND-LOOP STRUCTURES) by base-pairing between
complementary regions of the same molecule.
RNA (double- or single-stranded) constitutes the genome in
various ANIMAL VIRUSES, BACTERIOPHAGES and PLANT VIRUSES. In
prokaryotic and eukaryotic cells the major RNAs are involved
in all stages of PROTEIN SYNTHESIS (see MRNA, RRNA, TRNA),
and many other types of RNA play regulatory, catalytic or
other roles: see e.g. ANTISENSE RNA, RIBOZYME, SCRNA, SIGNAL
RECOGNITION PARTICLE, SNRNA.
RNA I See COLE1 PLASMID.
RNA II See COLE1 PLASMID.
RNA III See AGR LOCUS.
RNA blotting See BLOTTING.
RNA degradosome See DEGRADOSOME.
RNA-dependent DNA polymerase Syn. REVERSE TRANSCRIPTASE.
RNA editing In animals, plants and certain microorganisms: an
in vivo mechanism which can generate new functional transcripts
from existing ones. One (mammalian) example is the editing of
the mRNA for apolipoprotein B (apoB) by cytidine deaminase
(an enzyme which converts C to U); the unedited mRNA yields
a product of 4536 amino acids, while the edited mRNA (which
contains an internal stop codon formed by cytidine deaminase)
yields a product of 2152 amino acids.
Studies have suggested that RNA editing may be involved
in the differentiation/maturation of antigen-stimulated B cells in
germinal centres a period of development that includes affinity
maturation and class switching (see ANTIBODY FORMATION).
Thus, a deficiency in activation-induced cytidine deaminase
(AID) an enzyme found specifically in germinal centre B
cells has been found to inhibit both affinity maturation and
class switching [Cell (2000) 102 553563].
Deficiency in the AID enzyme has also been reported to
be responsible for the autosomal recessive form of hyper-IgM
RNase F
Eukaryotic nuclear RPases are not inhibited by rifamycins or
streptolydigin (cf. a-AMANITIN).
RPases from mitochondria and chloroplasts are distinct from
the nuclear enzymes, being e.g. much smaller.
The RPases of members of the ARCHAEA (formerly Archaebacteria) appear to be much more closely related to those
of the eukaryotic nucleus than to the bacterial enzyme;
they contain many components, and are relatively insensitive
to rifamycins, streptolydigin and a-amanitin. [Archaebacterial
(archaeal) RPases: Book ref. 157, pp. 499524.]
Some bacteriophages encode their own RPases; those of e.g.
T3 and T7 each consist of a single polypeptide chain. (See
also BACTERIOPHAGE N4 and BACTERIOPHAGE SP6.) In some cases
a phage modifies (and alters the specificity of) its hosts RNA
polymerase: see e.g. BACTERIOPHAGE T4 and BACTERIOPHAGE SPO1.
RNA splicing See SPLIT GENE.
RNA thermometer See HEAT-SHOCK PROTEINS.
RNA tumour viruses Viruses of the ONCOVIRINAE.
RNAase See RNASE.
RNAi See RNA INTERFERENCE.
RNAP RNA POLYMERASE.
RNase (RNAase; ribonuclease) An enzyme which cleaves RNA.
An RNase may be an ENDONUCLEASE (= endoribonuclease) or
an EXONUCLEASE (= exoribonuclease); enzymes in the latter
category may act randomly (dissociating from the substrate after
each catalytic event) or processively (see PROCESSIVE ENZYME).
A given RNase generates 3 -hydroxyl and 5 -phosphate or
3 -phosphate and 5 -hydroxyl termini. Most RNases rely on
the conformation of the RNA substrate (rather than nucleotide
sequence per se) for their specificity (cf. RNASE E).
RNases have important roles in RNA processing (see e.g.
MRNA, RRNA, TRNA), in certain types of regulatory process (e.g.
RETROREGULATION), and in degrading RNA molecules which
have fulfilled their function.
For examples of RNases see following entries.
RNases can be inactivated by DIETHYLPYROCARBONATE.
RNase See MRNA (a).
RNase I In Escherichia coli : an endoribonuclease (see RNASE)
which can degrade most RNA molecules to oligonucleotides
with 3 -phosphate and 5 -hydroxyl termini.
RNase II In Escherichia coli : an exoribonuclease (see RNASE)
which removes nucleoside 5 -phosphate residues from the 3 end
of an RNA molecule which has little or no secondary structure.
RNase III In Escherichia coli : an endoribonuclease (see RNASE)
which cleaves double-stranded regions in RNA molecules.
RNase III is involved in rRNA precursor processing (see RRNA),
in the RETROREGULATION of int gene expression in BACTERIOPHAGE LAMBDA, and in the release of monocistronic mRNAs from
the polycistronic early-gene transcript in BACTERIOPHAGE T7; the
target sites for RNase III action typically occur in stem-and-loop
or hairpin structures in the RNA.
RNase BN See TRNA.
RNase D See TRNA.
RNase E In Escherichia coli : an endoribonuclease (see RNASE)
which is involved e.g. in the formation of 5S rRNA from prerRNA (see RRNA). RNase E also cleaves RNA I (involved in the
replication of the COLE1 PLASMID and related plasmids), cleavage
occurring between the 5th and 6th nucleotides from the 5 end
of the molecule. The cleavage site occurs in a sequence of 10 nt
which is almost identical in the two RNA substrates [JMB (1985)
185 713720].
(See also DEGRADOSOME.)
RNase F See INTERFERONS.
RNase H
Rocio virus See FLAVIVIRIDAE.
rock tripe Umbilicaria spp, or the edible species U. esculenta
eaten (as iwatake) in Japan.
rocket immunoelectrophoresis (electroimmunoassay) IMMUNOELECTROPHORESIS in which (typically) antibody, at or near its
isoelectric point, is uniformly distributed in a gel layer, and
homologous antigen (in a well in the layer) is subjected to an
electric field. Antigen moves towards one of the poles, and forms
(with the antibody) a rocket-shaped line of precipitate an
extended paraboloid with the wide end towards the well; the
length of the rocket is proportional to the initial concentration
of antigen in the well.
Rocky Mountain spotted fever A rickettsial disease of man
which occurs in parts of North America, particularly in late
spring and summer; the causal agent, Rickettsia rickettsii, is
transmitted by ticks chiefly species of Dermacentor. Infection,
by the bite of an infected tick, is followed by an incubation
period of 214 days; symptoms include headache, joint and
muscular pains, and a sustained fever. A rash develops on
the limbs and trunk (in that order); the lesions may become
haemorrhagic and necrotic. Mortality in untreated cases may be
590%. Reservoirs of infection occur e.g. in the dog (which can
develop clinical signs) and in wild rodents. Lab. diagnosis: e.g.
a CFT and/or the WEILFELIX TEST.
rod (bacteriol.) Syn. BACILLUS sense 2.
rod organ (pharyngeal rod organ) See PERANEMA.
.
roentgen See RONTGEN
roestelioid (cornute) Refers to an elongated aecium which
projects through the epidermis of the host; at maturity the
exposed portion of the peridium typically ruptures by a number of longitudinal slits, the torn strips of peridium often curling
back in a rosette-like pattern. Such aecia are formed e.g. by
species of Gymnosporangium.
rofecoxib See PROSTAGLANDINS.
roguing (plant pathol.) The removal of diseased plants from a
crop in order to (e.g.) prevent the spread of the disease.
Rohament P A commercial PECTIC ENZYME preparation consisting mainly of endopolygalacturonase.
Rohr See PLASMODIOPHOROMYCETES.
roll-tube technique (Hungate technique; syn. Virginia Polytechnic
Institute (VPI) technique) A technique used for the isolation,
culture and enumeration of strict, O2 -sensitive ANAEROBES. Prereduced, agar-based media are sterilized in tubes, under anaerobic
conditions, and the processes of inoculation, incubation and
subculture are also carried out anaerobically; anaerobic conditions
are maintained within the tube during e.g. inoculation by inserting
a sterile cannula into the tube and passing in a gentle stream
of O2 -free gas (e.g. CO2 ) during any period when the tube is
unstoppered. For inoculation, the medium is melted, cooled to
ca. 45 C, and mixed with the inoculum; the tube is then held
horizontally and rotated about its long axis so that the agar
solidifies in a thin layer around the inner surface of the tube. The
tube is then incubated until individual colonies develop on and
within the medium. (If a heat-labile reducing agent is used in the
medium it is incorporated immediately prior to inoculation.)
roller culture In TISSUE CULTURE, a method of incubating bottles
and other vessels of circular cross-section: the culture vessels are
placed on a horizontal array of parallel, closely spaced rotating
rollers such that each vessel rotates about its long axis; during
incubation a monolayer develops as a continuous band on the
vessels inner surface. Culture vessels may be rotated at ca.
0.13.0 r.p.m. on commercially available apparatus. Benefits of
roller culture include a more efficient use of culture vessels, and
the various advantages of a continually mixed medium.
root nodules
[Book ref. 55, pp. 331, cf. pp. 116119]. Attachment may
be followed by a tight curling of the root hair tip (due to
differential cell wall synthesis in the root hair), resulting in
the formation of a pocket which encloses the bacteria. The
bacteria then penetrate the root hair via a tubular infection thread
which, originating at the site of infection, grows to the base of
the root hair and penetrates the underlying cortex. [Infection
process: ARM (1983) 37 399424.] The wall of the infection
thread seems to be of plant origin, resembling the primary plant
cell wall in composition; mucopolysaccharide (apparently of
bacterial origin) in the lumen may serve to protect the invading
bacteria from the hosts defence mechanisms [Book ref. 55,
pp. 5893]. The infection thread ramifies extensively within the
cortex, and cortical cells ahead of it proliferate apparently
in response to a diffusible substance(s) (?phytohormones).
(Rhizobia can produce IAA and cytokinins in vitro, but the
significance of this in nodule formation is unclear.) The
invading bacteria are released from the tips of the ramifying
infection thread into the proliferating cortical cells, within
which they undergo morphological and other changes to become
pleomorphic bacteroids enveloped in a membrane of plant origin
(the peribacteroid membrane). Once infected, host cells cease to
divide and begin to swell; they remain vacuolated. Cells beyond
the infection zone continue to divide until they too are invaded;
thus, throughout the development of the nodule there is an
advancing zone of meristematic cells. The bacteroid-containing
cells contain LEGHAEMOGLOBIN and form a pink zone between
the white zones of the meristem and of the ramifying infection
thread. In indeterminate nodules the fixed nitrogen is exported
from the nodule to the rest of the plant mainly as asparagine.
Determinate nodules occur in certain tropical legumes, soybeans, cowpeas etc. Infection threads enter the root cortex from
an infected root hair but do not ramify extensively after entering
the cortex; bacteria are spread mainly by division of infected
cortical cells. The nodules are spherical, with a cortical cell
layer surrounding a central, pink-pigmented zone containing
both infected and non-infected cells; the meristematic stage is
transient, restricted to the initial stage of nodule development.
Infected cells are not vacuolated, and the bacteroids are (nonpleomorphic) rods and swollen rods which divide to form up
to ca. 16 bacteroids within the peribacteroid membrane. Fixed
nitrogen is exported from the nodule as ureides (mainly allantoin
and allantoic acid).
An alternative infection strategy occurs in e.g. the peanut
(Arachis hypogea): bacteria enter the root at the junction
between the root hair and epidermal cells (crack entry), and
an infection thread is not formed. Interestingly, crack entry
has been exploited in the experimental infection of wheat
with the nitrogen-fixing bacterium Azorhizobium caulinodans;
A. caulinodans became established within the xylem and root
meristem such that experimental plants showed significantly
increased dry weight and nitrogen content in comparison to
uninoculated control plants [Proc. RSLB (1997) 264 341346].
Nodulation involves coordinated expression of plant and
bacterial genes, with derepression of certain plant genes (see
e.g. NODULINS) and bacteroid genes (e.g. NIF GENES). (See
also LEGHAEMOGLOBIN.) In Rhizobium spp many of the genes
involved in the initiation of root hair infection, nodule formation,
and nitrogen fixation are located on a large plasmid (Sym
plasmid ), although chromosomal genes are also involved (at
least in nitrogen fixation). Sym plasmids may code for additional
functions such as bacteriocin production, plasmid transfer,
pigment production, etc. Sym plasmids appear not to occur
rootlet
lambs, mice and piglets. (See also FOOD POISONING (i) and
Rotaviruses replicate in the
intestinal epithelial cells; the faeces of infected individuals may
contain up to e.g. 109 1010 virions per gram.
A serological classification system for rotaviruses was proposed in 1985 [Ann. Vir. (1985) 136 E 512]. Vaccination has
been used against rotavirus infection [see e.g. JID (1986) 153
815822, 823831 and 832839]; however, the tetravalent vaccine was withdrawn in 1999 (owing to side-effects), so that there
is currently no vaccination available against rotavirus infections.
The capsid of the rotavirus virion is icosahedral in shape and
is triple-layered, the outermost layer being lost during entry of
the virion into a host cell. The capsid comprises various types
of polypeptide the innermost layer consisting of 120 copies of
the VP2 protein, while the adjacent (middle) layer consists of
260 trimers of VP6.
The rotavirus genome consists of 11 dsRNA molecules.
Inside infected cells the double-layered viral particles become
transcriptionally active, mRNAs passing out through pores in
the capsid. VP6 is necessary for trancription, but its exact role is
unknown. The crystal structure of VP6 from a group A rotavirus
resolution; the results suggest that,
has been determined to 2 A
during assembly of the capsid, the addition of the VP6 layer
begins with the binding of VP6 trimers to the inner layer at the
20 icosahedral three-fold axes [EMBO (2001) 20 14851497].
(See also PARAROTAVIRUSES.)
rotenone A mitochondrial RESPIRATORY INHIBITOR which inhibits
electron flow between the FeS centres of Complex I and
ubiquinone (see ELECTRON TRANSPORT CHAIN); it binds, noncovalently, to a site which is apparently close to that at which
ubiquinone is reduced. Many bacterial systems are insensitive to
rotenone.
Rothia
A genus of aerobic, facultatively anaerobic, catalasepositive, asporogenous bacteria (order ACTINOMYCETALES, wall
type VI) which occur e.g. in the human mouth. The organisms
form a rudimentary mycelium which fragments into non-motile
rods and coccoid forms, the latter being ca. 15 m in diameter.
Growth occurs on rich media, e.g. trypticasesoy agar, at 37 C;
no growth occurs on Sabourauds dextrose agar. Various sugars
can be fermented; glucose metabolism yields mainly lactic
acid. GC%: ca. 6570. Type species: R. dentocariosa. [Strain
differentiation in R. dentocariosa: IJSB (1984) 34 102106.]
Rotorod An instrument used e.g. for sampling the airborne
microflora. (See also AIR.) Essentially, two vertically-orientated
adhesive- or grease-coated rods, at opposite ends of a horizontal
bar, are whirled at ca. 2500 rpm; the rods may be detached and
examined e.g. by microscopy.
rotund body See THERMUS.
rough endoplasmic reticulum See ENDOPLASMIC RETICULUM.
rough strain See SMOOTHROUGH VARIATION.
Rous-associated viruses See AVIAN LEUKOSIS VIRUSES.
Rous sarcoma virus (RSV) An AVIAN SARCOMA VIRUS originally
isolated from a naturally occurring sarcoma of a chicken;
when inoculated into chickens or other fowl, RSV can cause
sarcomas and a fatal acute erythroblastic leukaemia within 23
weeks. There are several strains of RSV which differ e.g.
in oncogenicity, host range, etc. Most strains are replicationdefective; all carry the ONCOGENE v-src (see SRC). Some strains
can induce tumorigenesis on inoculation into mammals (e.g.
mice, rabbits, monkeys). RSV can be cultivated in chick embryo
cells or in embryonated eggs defective strains requiring the
presence of an appropriate helper virus (Rous-associated virus:
see AVIAN LEUKOSIS VIRUSES).
676
RTF
routine test dilution (RTD) The highest dilution of a virus
suspension (i.e. the lowest concentration of viruses) which can
bring about confluent lysis in a monolayer of sensitive cells or
(in the case of bacteriophage) in a lawn plate prepared with a
sensitive strain of bacteria.
Roux flask (Roux bottle) A flat-sided, rectangular, glass or
plastic vessel which opens at one end via a short wide tube;
it is used, on its side, for TISSUE CULTURE.
roxithromycin A MACROLIDE ANTIBIOTIC.
Royce indicator sachet See ETHYLENE OXIDE.
Rozella See CHYTRIDIALES and MYCOPARASITE.
RP 59500 See QUINUPRISTIN/DALFOPRISTIN.
RP1 b-lactamase Syn. TEM-2 b-LACTAMASE.
RP1 plasmid (syn. R1822 plasmid) A CONJUGATIVE PLASMID
(COPY NUMBER: 12) which occurs in both enterobacteria and
Pseudomonas spp (IncP/IncP-1); it encodes resistance to carbenicillin, kanamycin and tetracycline. Plasmids R18, R68, RK2
and RP4 are very similar or identical to RP1.
RP4 plasmid See RP1 PLASMID.
RPase RNA POLYMERASE.
RPCF test See TREPONEMAL TESTS.
RPG effect The phenomenon (discovered by R. P. Gunsalus) in
which METHANOGENESIS from CO2 and H2 (in crude extracts of
certain methanogens) is stimulated by methyl-coenzyme M.
rpl genes
Genes encoding r-proteins of the large ribosomal
subunit: see RIBOSOME.
rpo genes
Genes which encode DNA-dependent RNA POLYMERASE subunits; in e.g. Escherichia coli, rpoA, rpoB, rpoC
and rpoD encode subunits a, b, b , and the major SIGMA FACTOR, respectively. [Autogenous control of rpo genes: Genet. Res.
(1986) 48 6164.] (See also RIBOSOME (biogenesis).)
rpoB gene In Mycobacterium tuberculosis: a gene encoding the
b subunit of RNA polymerase. Mutations in rpoB are associated
with resistance to the drug rifampicin; such mutations are
detected by various genotypic methods which are used for testing
isolates of M. tuberculosis for resistance to rifampicin for
further details see SSCP, PROBE and TUBERCULOSIS.
rpoH gene (htpR gene) See HEAT-SHOCK PROTEINS.
rpoN gene See NTR GENES.
rpoS gene See SIGMA FACTOR.
RPR test Rapid plasma reagin test: a qualitative or quantitative
STANDARD TEST FOR SYPHILIS in which the cardiolipinlecithin
cholesterol antigen is modified by the incorporation of choline
chloride; this modification permits serum to be tested without
prior heating (cf. VDRL TEST). In the RPR (circle) card test the
antigen suspension contains particles of charcoal; this permits
flocculation to be assessed macroscopically. (cf. RST.)
rps genes
Genes encoding r-proteins of the small ribosomal
subunit: see RIBOSOME.
rrn operons See RRNA and RIBOTYPING.
rRNA Ribosomal RNA: the major component of a RIBOSOME (q.v.
for structure etc). In e.g. Escherichia coli rRNA is encoded
by 7 separate operons (designated rrnA to rrnG), each of
which is transcribed (see TRANSCRIPTION) to give a single RNA
precursor molecule (pre-rRNA, ca. 30S) which contains all three
rRNA species. An rrn operon has two promoters (P1 and P2)
separated by 109119 bp, and has the overall structure: P1P2-leader16S rRNA genespacer23S rRNA gene5S rRNA
geneterminator; one or two tRNA genes lie in the transcribed
spacer between the 16S and 23S rRNA genes, and in some
cases one or two tRNA genes also occur at the 3 (distal) end
of the operon.
The 30S pre-rRNA contains internal inverted repeats which
can base-pair to form secondary structures. The 16S and 23S
rRNA sequences each form the loop in a separate stem-andloop structure, and are released from the pre-rRNA by the
endoribonuclease RNASE III; RNase III makes a staggered break
in each of the double-stranded stem regions to liberate individual
16S and 23S rRNA precursors (designated p16S and p23S)
which are slightly longer than the mature molecules. The RNase
III cleavage sites show no homology; the enzyme presumably
recognizes secondary and/or tertiary structure in the RNA.
Subsequent processing of the individual precursors to form the
mature rRNA molecules is not well understood; that of the 5S
rRNA involves the endonuclease RNASE E. (For processing of the
tRNA(s) see TRNA.)
Because rRNA genes are transcribed but not translated, they
might be expected to show a high incidence of premature
transcription termination owing to the absence of the protective
effect of ribosomes (see POLAR MUTATION). Apparently, specific
ANTITERMINATION mechanisms operate in the rrn operons of
E. coli : modification of the RNA polymerase as it transcribes
certain sequences in the rrn leader region may occur, allowing
the polymerase to continue transcription until it reaches a strong
rrn terminator [minireview: JB (1986) 168 15].
Eukaryotes synthesize an rRNA precursor (ca. 45S) which
contains a leader sequence and sequences for the 28S, 18S, and
5.8S rRNAs separated by transcribed spacers; 45S transcripts are
transcribed from many tandemly repeated sets of genes separated
by non-transcribed spacer sequences. The 45S precursor is synthesized by RNA polymerase I in the NUCLEOLUS [minireview:
Cell (1986) 47 839840]; the 5S rRNA genes are organized
separately and are transcribed by RNA polymerase III. (In certain lower eukaryotes e.g. in Dictyostelium discoideum, and
in the macronucleus of Tetrahymena rRNA genes occur on
extrachromosomal DNA molecules present in many copies per
nucleus.) (See also SPLIT GENE (b).)
rRNA oligonucleotide cataloguing A procedure once used in
bacterial TAXONOMY. Essentially, rRNA (usually 16S rRNA) is
cleaved by a sequence-specific endonuclease (e.g. RNase T1);
the fragments are end-labelled, separated by electrophoresis, and
then sequenced giving a catalogue of sequences characteristic of the species. The catalogues of various species can then
be compared and used as a basis for classification. [16S rRNA
oligonucleotide cataloguing: Book ref. 138, pp 75107.]
rRNA oligonucleotide cataloguing was one of the earlier
methods used in molecular taxonomy. Subsequently, more informative methods (e.g. sequencing of the entire rRNA molecule)
were developed.
rRNA superfamily VI See HELICOBACTER.
RS layer Syn. S LAYER.
Rsd protein See ANTI-SIGMA FACTOR.
RSF1010 plasmid See INCOMPATIBILITY.
RSF1030 plasmid See COLE1 PLASMID.
RSSE RUSSIAN SPRINGSUMMER ENCEPHALITIS.
RST Reagin screen test: a qualitative or quantitative STANDARD
TEST FOR SYPHILIS in which the antigen has been dyed blue in
order to permit macroscopic assessment of flocculation (cf. RPR
TEST).
RSV (1) Respiratory syncytial virus. (2) Rous sarcoma virus.
Rta See ZEBRA.
RTD ROUTINE TEST DILUTION.
RTEM b-lactamase Syn. TEM-1 b-LACTAMASE.
RTF (1) Resistance transfer factor: that part of a conjugative R
PLASMID which contains the genes specifying CONJUGATION; thus,
a conjugative R plasmid consists of the RTF together with the
gene(s) encoding resistance (resistance determinants). The RTF
is usually self-repressed. (See also SEX FACTOR.)
677
rtPCR
rubella (German measles) (1) An acute infectious human disease, which affects mainly children and young adults, caused
by a virus (see RUBIVIRUS).
Acquired rubella. Infection occurs by droplet inhalation. Incubation period: 23 weeks. Early symptoms may include mild
upper respiratory tract symptoms, mild fever, and enlargement
of the lymph nodes of the head and neck. Following a stage of
viraemia, a maculopapular rash appears first on the face, then
on the rest of the body. Patients are infectious for ca. 1 week
before and ca. 1 week after the onset of symptoms. The disease is usually mild and self-limiting; occasional complications
include e.g. arthritis and encephalitis.
Congenital rubella. Maternal rubella acquired during pregnancy can lead to a persistent infection of the fetus and neonate,
resulting in teratogenic effects which may range from mild (e.g.
low birth weight) to fetal death; intermediate manifestations
include permanent defects in the CNS (e.g. mental retardation),
ears (nerve deafness), eyes (e.g. cataracts, retinal damage), heart
etc (cf. TORCH DISEASES). Damage is most severe if infection
is acquired during the first 3 months of pregnancy. A progressive rubella panencephalitis resembling SUBACUTE SCLEROSING
PANENCEPHALITIS has been reported as a late manifestation of
congenital rubella [NEJM (1975) 292 990993, 994998].
Lab. diagnosis: detection of rubella-specific antibodies e.g. by
a haemagglutination-inhibition test, radial haemolysis, ELISA
etc. Rubella virus can be isolated from e.g. nasopharyngeal
swabs. Prophylaxis: vaccination with a live, attenuated vaccine
(see also MR and MMR).
(2) Syn. INFECTIOUS DROPSY (of carp).
rubelliform Refers to a RUBELLA-like disease or rash.
rubeola (1) (English, German) Syn. MEASLES. (2) (French, Spanish) Syn. RUBELLA.
rubidomycin See ANTHRACYCLINE ANTIBIOTICS.
RuBisCO RIBULOSE 1,5-BISPHOSPHATE CARBOXYLASEOXYGENASE.
Rubivirus
A genus of viruses (family TOGAVIRIDAE) which
currently includes only the RUBELLA virus. Man is apparently the
only natural host; some laboratory animals can be infected, but
none develops a disease analogous to that in man. (There is no
invertebrate host.) The rubivirus virion is relatively unstable at
room temperatures, loses infectivity within ca. 30 min at 56 C,
but is stable for ca. 1 week in protein-containing solutions at
4 C; it can be stored at or below 60 C, and can withstand
freeze-drying. It can be inactivated by pH <6.8 or >8.1, by
organic solvents, UV radiation, deoxycholate, ethylene oxide,
etc. The virions promote Ca2+ -dependent haemagglutination of
RBCs from various species (those from newly hatched chick,
adult goose or pigeon, or human O-type RBCs being commonly
used in HI tests). Rubella virus can grow in various types
of cell culture; primary African green monkey kidney cells
have been widely used for primary isolation. The virus is noncytopathogenic in most vertebrate cells, and can be detected
e.g. by immunofluorescence techniques and by its ability to
prevent the replication of a superinfecting challenge virus such
as echovirus type 11 (see INTERFERENCE). [Clinical aspects: Book
ref. 148, pp. 10051020.]
RuBP Ribulose 1,5-bisphosphate.
RuBPCase See RIBULOSE 1,5-BISPHOSPHATE CARBOXYLASEOXYGENASE.
rubratoxins MYCOTOXINS produced e.g. by strains of Penicillium rubrum; toxin production is associated with active fungal
growth. Consumption of rubratoxins by animals causes congestion of tissues (often with haemorrhage) especially in the
stomach and intestine; liver damage and brain lesions can also
occur. Rubratoxins and AFLATOXINS act synergistically.
rumen
rubredoxins See IRONSULPHUR PROTEINS.
Rudimicrosporea A class of protozoa (phylum MICROSPORA)
which are hyperparasites of gregarines in annelid worms. The
spores have a simple (rudimentary) extrusion apparatus consisting of a polar cap and thick polar tube terminating in a funnel
(the infundibulum). There is no polaroplast. Genera: e.g. Amphiacantha, Metchnikovella.
rugose Wrinkled.
rugose mosaic disease (1) The disease of potatoes caused by
POTATO VIRUS Y (Yo strains) in the second and subsequent years
of infection. (2) A severe disease of potatoes caused by mixed
infection with potato virus X and POTATO VIRUS Y (Yo strains).
rule of desmodexy (ciliate protozool.) The rule, based on observation, that each kinetodesma lies on the right-hand side of its
corresponding kinetosome: see KINETODESMA.
rum See SPIRITS.
rumen One of four compartments which form the stomach in
ruminants (cattle, deer, giraffes, goats, sheep etc); the other
compartments are the reticulum (an outpocketing of the rumen
usually included with the rumen proper when reference is
made to the rumen), the omasum, and the abomasum or true
stomach.
In the adult or weaned ruminant, food passes from the
oesophagus to the rumen. The rumen (capacity ca. 510
litres in sheep, 100150 litres in cattle) is essentially an
anaerobic muscular sac which contains a large population
of microorganisms (on average ca. 1010 cells/ml) primarily
bacteria and protozoa, but sometimes including a significant
proportion of fungi; these microorganisms play an essential role
in ruminant nutrition by breaking down the ruminants diet
of plant material (see ANAEROBIC DIGESTION) and providing the
animal with assimilable nutrients and sources of energy. (The
microflora of the rumen is indispensable to the ruminant since
many of the components of plant material are not attacked by the
enzymes of animal digestive systems. The rumen itself does not
secrete enzymes.) To allow adequate time for microbial action,
large particles of food may remain in the rumen for several
days. Periodically a bolus of partly digested material (a cud ) is
regurgitated to the mouth, chewed, and swallowed; cuds return
to the rumen where they undergo further digestion. The net
effect of digestion in the rumen is the conversion of dietary
materials to a mixture of fatty acids (mainly acetic, butyric and
propionic acids), gases (primarily CO2 and CH4 which are
voided by eructation), and microbial biomass. Fatty acids are
absorbed by the rumen and are used by the ruminant as primary
sources of carbon and energy. Microbial biomass passes from
the rumen to the omasum where residual fatty acids, water
and salts are absorbed and then to the abomasum where the
biomass undergoes true (gastric) digestion; digested material
passes into the small intestine where it is absorbed by the
ruminant amino acids derived from the digestion of microbial
protein constituting the principal source of nitrogen for the
ruminant. Certain vitamins synthesized by the rumen bacteria
(e.g. VITAMIN B12 ) are also absorbed as the rumen contents pass
through the abomasum and intestines.
Ruminants produce large amounts of saliva; the saliva contains bicarbonate and phosphate which buffer the rumen contents maintaining a pH of ca. 6.06.5 despite the ongoing
formation of acidic products by microbial fermentations. The
temperature of the rumen (in the cow) is ca. 3940 C, slightly
higher than the body temperature (ca. 38 C) due partly to the
exothermic microbial metabolism. The Eh of the rumen has been
reported to be in the range 145 mV to 260 mV. [Influence
rumenitis
to the rumen (via the rumen wall, or in the saliva); here, the
urea is cleaved by microbial ureases and the resulting ammonia
is incorporated into microbial biomass. Thus, dietary nitrogen
is conserved, and ruminants can survive on low-nitrogen diets.
Feedstuffs low in nitrogen can be supplemented with e.g. urea.
In the suckling ruminant the rumen is poorly developed; milk
passes from the oesophagus, via the oesophageal groove, directly
to the omasum and abomasum (i.e., by-passing the rumen)
and is digested by processes similar to those in other young
mammals; the intestinal flora includes species of Lactobacillus
and Streptococcus.
[Review of microbial ecology and activities in the rumen:
CRM (1982) 9 165225 (part I) and 253320 (part II).]
rumenitis Inflammation of the RUMEN. Primary rumenitis, involving erosion of the rumen wall, can occur as a result of ACIDOSIS; the weakened rumen wall may subsequently be invaded by
pathogenic microorganisms which may give rise e.g. to necrotic
foci in the rumen and/or in other tissues (such as the liver).
rumensin Syn. MONENSIN.
ruminal Of or pertaining to the RUMEN.
ruminal tympany Syn. BLOAT.
ruminate (1) (verb) To chew the cud. (See also RUMEN.)
(2) (adj.) Much folded as though having been chewed.
Ruminococcus A genus of GRAM TYPE-positive, asporogenous,
anaerobic, typically cellulolytic bacteria which occur e.g. in
the RUMEN; GC%: ca. 4045. Cells: cocci (ca. 1 m diam.)
which occur in pairs or chains. Metabolism is typically heterofermentative; the main products of carbohydrate metabolism
include acetic and formic acids (lactic acid may be formed in
small amounts). CELLOBIOSE and (commonly) CELLULOSE are fermented; glucose and other simple sugars may or may not be
fermented, according to strain (many strains lack a glucose transport system). Ammonia is essential as a source of nitrogen for
most or all strains. Other growth requirements may include e.g. B
vitamins. Type species: R. flavefaciens. Other species: R. albus.
RuMP pathway Syn. RMP PATHWAY.
rumposome In zoospores of certain members of the CHYTRIDIOMYCETES (e.g. Monoblepharella): a body of unknown function
(though thought to be light-sensitive) which occurs beneath the
cytoplasmic membrane at the posterior end of the cell.
Runella A genus of pink-pigmented bacteria (family SPIROSOMACEAE). The cells, 0.50.9 2.04.5 m, are typically moderately or strongly curved the ends of curved cells sometimes overlapping to form ring-shaped structures. Acid is
formed from few carbohydrates. GC%: 4950. Type species:
R. slithyformis.
Runyon groups In the genus Mycobacterium: groups of species
distinguished on the basis of growth rate and pigmentation; slowgrowing species are placed in groups I (photochromogens), II
(scotochromogens), and III (others), while fast-growing species
are placed in group IV.
Russian autumn encephalitis Syn. JAPANESE B ENCEPHALITIS.
Russian flu See INFLUENZAVIRUS.
Russian springsummer encephalitis (RSSE) An acute human
ENCEPHALITIS caused by a flavivirus (see FLAVIVIRIDAE); it occurs
in epidemics, chiefly in and around the forests of Siberia. It is
transmitted by ticks (e.g. Ixodes sp); human infection can also
occur by ingestion of meat or milk from infected animals. The
disease varies from mild to fatal; encephalitis may be followed
by chronic progressive neuromuscular disorders or paralysis
months or years after the original infection, apparently due to
the persistence of the RSSE virus in the CNS. [ARE (1981) 26
8082.]
ryegrass staggers
Russian winter wheat mosaic virus See RHABDOVIRIDAE.
Russula A genus of fungi (family RUSSULACEAE) which form
mushroom-shaped, lamellate fruiting bodies that do not form
latex (cf. LACTARIUS). R. emetica is a poisonous species (the
sickener) which forms a fruiting body having a bright red, shiny
cap; it is commonly found under or near pine trees. R. mairei
(the beechwood sickener) is another red-capped, poisonous
species found near beech trees.
Russulaceae A family of fungi (order RUSSULALES) which form
ballistospores on stipitate, agaricoid to gasteroid fruiting bodies.
Genera include LACTARIUS and RUSSULA.
Russulales An order of fungi (subclass HOLOBASIDIOMYCETIDAE)
in which a characteristic feature is the presence of SPHAEROCYSTS
in the tissues of the fruiting body. The two families are
Elasmomycetaceae (members form statismospores in gasteroid
fruiting bodies) and RUSSULACEAE. (See also GASTEROMYCETES
(Hymenogastrales) and SECOTIOID FUNGI.)
rust See RUSTS.
rusticyanin A BLUE PROTEIN (MWt ca. 16500) which occurs in
681
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
S
s Sedimentation coefficient: see SVEDBERG UNIT.
S (1) SVEDBERG UNIT. (2) Serine (see AMINO ACIDS).
S fimbriae FIMBRIAE which occur on many of the strains of
Escherichia coli which cause meningitis in human neonates;
they bind to sialyl galactoside receptors on human erythrocytes.
S-glucan Alkali-soluble glucans of fungal CELL WALLS. (cf. RGLUCAN.)
s. lat. SENSU LATO (q.v.).
S layer In a prokaryotic cell: a continuous layer often the outermost layer of the cell consisting of a repeating pattern of protein or glycoprotein subunits (S proteins) arranged in squares,
hexagons etc. S layers occur in bacteria (including strains
of e.g. Aeromonas, Campylobacter, Clostridium, DEINOCOCCUS,
Lactobacillus, Nitrosomonas, Pseudomonas, Treponema, some
cyanobacteria) and archaeans (including strains of e.g. Desulfurococcus, Halobacterium, Methanococcus, Sulfolobus).
In bacteria, the S layer usually overlays the cell wall
proper e.g. in Gram-negative species it is external to the outer
membrane. A Bacillus sp with an S layer on both sides of the
cell wall has been reported [FEMS (1987) 40 7579]. Double
S layers, containing the same or different subunits, occur e.g.
in strains of Aquaspirillum, Bacillus and Corynebacterium. (See
also GLYCOCALYX.)
In a strain of Bacillus stearothermophilus it has been found
that variation in the S layer involves a chromosomeplasmid
re-arrangement of DNA [JB (2001) 183 16721679].
In some archaeans the S layer is the only cell wall component,
being immediately external to the cytoplasmic membrane.
S proteins are typically rich in acidic residues. In Gramnegative bacteria the S proteins interact with LPS in at least
some cases by non-covalent links; changes in composition of
LPS have been associated with the loss of an S layer. The
mRNAs of S protein genes are typically long-lived (1020
minutes).
S proteins typically have an N-terminal signal peptide, indicating secretion by a type II (sec-dependent) system (see PROTEIN
SECRETION). However, the way in which these proteins aggregate to form an S layer, and their mode of binding to LPS in
Gram-negative bacteria, is not understood.
[Review: ARM (1983) 37 311339. Principles of S layer
organization: JMB (1986) 187 251253. Secretion of S layers
in Gram-negative bacteria: FEMS Reviews (2000) 24 2144
(3538).]
S matrix In NUMERICAL TAXONOMY, similarity matrix: the percentage similarity between each OTU and each of every other
OTU (in a given study) expressed in tabular form the ordinate
and abscissa of the matrix each comprising a complete list of
designations of the OTUs under study.
S organism See METHANOBACILLUS OMELIANSKII.
S phase (of cell cycle) See CELL CYCLE.
S protein (immunol.) A protein (MWt ca. 80000) found in normal
plasma. S protein binds to the fluid-phase (i.e. non-membranebound) complex C5b67 formed during COMPLEMENT FIXATION,
destroying its membrane-binding and haemolytic potential. (See
also REACTIVE LYSIS.)
SR variation See SMOOTHROUGH VARIATION.
S ring See FLAGELLUM (a).
s. str. SENSU STRICTO (q.v.).
S strain See SMOOTHROUGH VARIATION.
Saccharomycetaceae
The vegetative cells are normally predominantly diploid (or
polyploid) predominantly haploid species having been placed
in the genera ZYGOSACCHAROMYCES and TORULASPORA. Asci,
which are persistent, develop directly from the diploid vegetative
cells. Ascospores are spheroidal, usually smooth, 14 per ascus.
Conjugation occurs on, or shortly after, germination of the
ascospores, i.e., it occurs between ascospores or between haploid
somatic cells derived therefrom. Species can ferment one or
more sugars, and can also carry out respiratory metabolism of a
range of substrates. NO3 is not assimilated. Seven species have
been recognized [Book ref. 100, pp. 379395]; type species:
S. cerevisiae.
S. cerevisiae (including many varieties and physiological races formerly accorded species status e.g. S. aceti,
S. carlsbergensis, S. diastaticus, S. ellipsoideus, S. globosus,
S. intermedius, S. inusitatus, S. sake, S. uvarum etc). Cells
(e.g. after 3 days at 25 C in malt extract) are ca. 310
420(30) m, occurring singly or in pairs, short chains or
clusters. (See also CELL WALL.) Pseudohyphae may be formed
e.g. on cornmeal agar. Many strains are heterothallic (see MATING TYPE). Sporulation is encouraged by media which are low
in nitrogen and which contain acetate as the main or sole carbon source. All strains can ferment glucose, some can ferment
galactose, sucrose and maltose, none can ferment lactose. (See
also ALCOHOLIC FERMENTATION.) In the presence of O2 , strains
can metabolize (oxidatively) substrates such as glycerol, ethanol
and lactate. All strains are sensitive to cycloheximide (100 ppm).
Strains have been isolated from e.g. alcoholic beverages, fruits
and fruit juices, soil, human skin and sputum, etc.
Selected strains of S. cerevisiae are widely used in the
manufacture of alcoholic beverages and fermented foods: see
e.g. BREAD-MAKING (and BAKERS YEAST), BREWING (and BREWERS YEAST), CIDER, KEFIR, PULQUE, SAKE, WINE-MAKING, YEAST
EXTRACT. (See also CHEESE-MAKING (c), IMMOBILIZATION (sense
1), STEROID BIOCONVERSIONS, WINE SPOILAGE.) S. cerevisiae is
also widely used in genetic studies and for the propagation
of genetically engineered genes. (See also e.g. KILLER FACTOR, KILLER PLASMIDS, TWO-MICRON DNA PLASMID, THREE-MICRON
DNA PLASMID.) [Genetic map of S. cerevisiae: MR (1985) 49
181212.]
S. dairensis (= S. castellii ). Cells (in malt extract): ca.
3.05.5 3.57.0 m, occurring singly or in pairs. Glucose
and galactose are fermented; sucrose, maltose and lactose are
not. Most strains can grow in the presence of cycloheximide at
100 ppm but not at 1000 ppm. Strains have been isolated from
buttermilk, soil and fermenting cucumber brines.
S. exiguus (anamorph: Candida holmii ). Cells (in malt
extract): ca. 2.55.0 3.56.5 m, occurring singly or in pairs.
Glucose, galactose and sucrose are fermented; maltose and lactose are not. Most strains can grow in the presence of cycloheximide at 100 ppm but not at 1000 ppm. Strains have been
isolated from soil, fruit, fermenting cucumber brines etc. (See
also BREAD-MAKING.)
S. kluyveri. Cells (in malt extract): ca. 3.57.0 4.011.0 m,
occurring singly or in pairs or clusters; pseudohyphae are usually
formed e.g. on cornmeal agar. Glucose, galactose and sucrose are
fermented, maltose and lactose generally are not, although some
strains can ferment maltose weakly. All strains are sensitive
to cycloheximide (100 ppm). The organisms closely resemble
S. cerevisiae but can be distinguished by their ability to grow
on ethylamine, cadaverine or L-lysine as sole nitrogen source.
Strains have been isolated from Drosophila spp, tree exudates,
soil, and fruit juice.
Saccharomycodes
is conducted through an open front panel or by means of armlength rubber gloves fitted into holes in the panel. The operator
and environment are given some protection, but cultures etc are
not. Class II cabinet. Sterile (filtered) air enters the cabinet and
passes downward onto the work surface; air (some of which may
be re-circulated) passes to the exterior via an exit port (situated
below the work surface) and is filtered before discharge to the
environment. Work is conducted via an open front panel; the
downward, laminar air-flow inside the cabinet, and the entry of
air via the front panel, together form a moving curtain of air
which helps to protect the user, the cultures etc. and the environment. Class III cabinet. Sterile, filtered air enters the gas-tight
cabinet, and air is filtered before discharge; a negative pressure is
maintained inside during use. Work is conducted via arm-length
rubber gloves fitted into the front panel. Access to the interior
of the cabinet is via a separate two-door sterilizing/disinfecting
chamber. [Book ref. 2, pp. 495499.]
safranin O A red basic composite azine DYE.
SAG Sammlung von Algenkulturen (algal culture collection),
Pflanzenphysiologisches, Universitat Gottingen, Gottingen, Germany.
SAg SUPERANTIGEN.
sagenogen See LABYRINTHULAS and THRAUSTOCHYTRIDS.
sagenogenetosome See LABYRINTHULAS and THRAUSTOCHYTRIDS.
Sagiyama virus See ALPHAVIRUS.
saguaro cactus virus See TOMBUSVIRUSES.
SAIDS SIMIAN AIDS.
saimiriine herpesvirus See e.g. GAMMAHERPESVIRINAE (Herpesvirus saimiri ).
Saint Anthonys fire (1) Syn. ERGOTISM. (2) Syn. ERYSIPELAS.
Saint Louis encephalitis See ST LOUIS ENCEPHALITIS.
Saint Vituss dance See RHEUMATIC FEVER.
sakacin A A 41-amino-acid, pore-forming class IIa BACTERIOCIN
produced by Lactobacillus sake; synthesis is reported to be
temperature-dependent and regulated by a three-component
system [Microbiology (2000) 146 21552160].
sake Japanese rice wine. Rice starch is degraded to fermentable
sugars by Aspergillus oryzae in a steamed rice KOJI; this is
inoculated with Saccharomyces sake, a strain of S. cerevisiae
with a high alcohol tolerance. A succession of organisms
follows A. oryzae: nitrate-reducing bacteria, followed by lactic
acid bacteria, followed by yeasts S. sake finally becoming
dominant [Book ref. 6, pp. 417419]. The alcohol content
reaches 20% v/v or higher.
Saksenaea See MUCORALES.
Saksenaeaceae See MUCORALES.
SAL plasmid An IncP-9 Pseudomonas PLASMID (ca. 85 kb)
which encodes the capacity to metabolize salicylate. (cf. TOL
PLASMID.)
SalI
A RESTRICTION ENDONUCLEASE from Streptomyces albus;
G/TCGAC.
salami Salami and salami-type sausages are manufactured by the
fermentation of comminuted meat (usually salted and spiced)
by (mainly) LACTIC ACID BACTERIA; traditional methods rely
on the microflora of the meat, equipment, environment etc,
but commercial starter cultures may be used. The product is
extremely resistant to microbial spoilage owing to its low pH
(usually ca. 4.85.2) and low aw (usually ca. 0.70.8); however,
it may be susceptible to spoilage by moulds and xerophilic
yeasts. The lactic acid bacteria contribute to the preservation
of salami by lowering the pH (by LACTIC ACID FERMENTATION
of carbohydrates) and e.g. by the production of antibiotics (see
FOOD PRESERVATION (e)); they also contribute to the flavour and
Salmonella
texture of the product. Some salami-type sausages are mouldripened, usually with Penicillium spp.
salicin 2-Hydroxymethylphenyl-b-D-glucopyranoside. It can be
hydrolysed by b-glucosidase to D-glucose and saligenin (2hydroxymethylphenol).
salicylanilides (as antimicrobial agents) Salicylanilide (2-hydroxy-N-phenylbenzamide) and its halogenated derivatives have
antifungal and antibacterial activity and are used e.g. as antiseptics and industrial PRESERVATIVES. Salicylanilide itself (Shirlan)
is used e.g. as an antifungal agent in textiles and wood pulps
and for the antifungal treatment of walls and ceilings; it has also
been used for the treatment of cutaneous mycoses.
salicylic acid (2-hydroxybenzoic acid) An antimicrobial, mildly
keratinolytic ORGANIC ACID used for the topical treatment of
e.g. ACNE and (with other agents) superficial mycoses. (cf.
SALICYLANILIDES.)
saligenin See SALICIN.
saline agglutination Syn. AUTO-AGGLUTINATION.
salinomycin An ionophore antibiotic, produced by Streptomyces
albus, which is used as an anti-coccidial agent in poultry and as
a FEED ADDITIVE for e.g. ruminants and pigs.
Salivaria One of two groups of subgenera of mammalian trypanosomes; salivarian trypanosomes infective for the vertebrate
host develop in the ANTERIOR STATION. The group comprises
DUTTONELLA, NANNOMONAS, PYCNOMONAS and TRYPANOZOON. (cf.
STERCORARIA.)
Salk vaccine An anti-poliomyelitis vaccine containing formalininactivated strains of three types of poliovirus; it is administered
intramuscularly. (cf. SABIN VACCINE.)
salmon disease See ULCERATIVE DERMAL NECROSIS.
salmon poisoning (in dogs) See NEORICKETTSIA.
Salmonella A genus of Gram-negative bacteria of the ENTEROBACTERIACEAE (q.v. for general features). Cells: straight rods,
ca. 0.51.0 15 m; most strains are motile. Reactions for
most salmonellae: indole ve; MR +ve; VP ve; citrate +ve;
acid and gas from glucose at 37 C; lactose usually ve; H2 S
+ve (in TSI); urease ve; lysine decarboxylase +ve; ornithine
decarboxylase +ve (cf. serotypes listed below). Reactions may
be altered e.g. by the presence of metabolic plasmids (e.g. a
plasmid carrying genes for lactose utilization [FEMS (1983)
17 127130]). Salmonellae can grow e.g. on NUTRIENT AGAR,
MACCONKEYS AGAR, and DCA, but usually not in KCN media.
685
Subspecies number
I
II
III(a)
III(b)
IV
V
VI
See text.
Subspecies I (enterica) contains the majority
of salmonellae pathogenic in man and warmblooded animals.
Salmonella/microsome assay
salvage pathway (complement fixation) See COMPLEMENT FIXATION (d).
salvarsan See ARSENIC.
same-sense mutation A POINT MUTATION in a structural gene
which results in a mutant codon specifying the same amino acid
as did the original codon (owing to the degeneracy of the GENETIC
CODE). (cf. SILENT MUTATION.)
San Joaquin Valley fever Syn. COCCIDIOIDOMYCOSIS.
San Miguel sea lion virus (SMSV) A virus (family CALICIVIRIDAE) isolated from sea lions (in which it may cause abortion)
and apparently widespread among marine mammals, fish etc in
the Pacific. SMSV is very closely related to vesicular exanthema
of swine virus, and can cause a disease similar to vesicular exanthema in pigs; it is only distantly related to FELINE CALICIVIRUS.
SMSV can be propagated e.g. in Vero cells.
sand filter See WATER SUPPLIES.
sandfly fever group See PHLEBOVIRUS.
sandwich technique A type of indirect IMMUNOFLUORESCENCE
technique used e.g. to demonstrate the presence of specific antibodies at the surface of antibody-forming cells. Essentially, a
suitably prepared section or smear is incubated with antigen
homologous to the given antibody, and subsequently washed
free of uncombined antigen; the preparation is then exposed
to a fluorescent antibody of the same specificity as that being
sought in the specimen, washed, and examined by fluorescence
MICROSCOPY. The antigen is thus sandwiched between homologous antibody in the specimen and homologous, fluorescent
antibody.
Sangers chain-termination method See DNA SEQUENCING.
sanitizer Any preparation with both cleansing and antimicrobial
properties (e.g. TEGO COMPOUNDS).
sap-stain Discoloration of freshly felled (moist) timber due to
growth of fungi primarily or solely in the sapwood; wood may
become e.g. green, purple or blackish, but more often appears
bluish-grey (see BLUE-STAIN). Sap-staining fungi include e.g.
Aureobasidium pullulans, Cladosporium herbarum, and species
of Diplodia and Graphium. (See also TIMBER PRESERVATION.)
sap transmission Transmission of a plant virus by a mechanical
VECTOR.
saponins A diverse group of powerful glycoside surfactants produced by a wide range of plants. Saponins have antifungal
properties which depend on their ability to affect membrane permeability by complexing with sterols in the CYTOPLASMIC MEMBRANE (see e.g. TOMATINE); certain bacteria (e.g. MYCOPLASMA
spp) can be lysed by saponins. (See also AVENACIN, BIOSURFACTANTS and DIGITONIN.)
saprobe Syn. SAPROTROPH.
saprobity system The system by which an organically polluted
river or stream undergoing SELF PURIFICATION may be divided into
a number of distinct zones, each zone being characterized e.g.
by its level of pollution, content of dissolved oxygen, and types
of microorganism (indicator-organisms) present. The polysaprobic zone is the zone most heavily polluted with organic matter
(sewage etc), i.e., the zone nearest the source of pollution. In
this zone oxygen consumption is high (dissolved O2 is minimal) and there is a vigorous production of ammonia and H2 S.
The organisms found in this zone may include e.g. the flagellates Bodo and Euglena, the ciliate Glaucoma scintillans, and
various bacteria such as Beggiatoa, Thiothrix and Oscillatoria.
In the a-mesosaprobic zone MINERALIZATION and oxygen consumption continue vigorously, but the content of dissolved O2
is higher than that in the polysaprobic zone; there is some in
situ utilization of ammonia, and there is no free H2 S. Organisms in this zone may include e.g. Oscillatoria, and the ciliates
Sarcodina
of decay and MINERALIZATION, and are thus essential links in the
cycles of matter (see e.g. CARBON CYCLE). Some saprotrophs are
facultative PARASITES. (cf. SAPROPHYTE; SAPROZOITE.)
saprotrophic (saprobic) Refers to a SAPROTROPH or to the mode
of nutrition of a saprotroph.
saprovore Syn. SAPROTROPH.
saprozoite An animal-like SAPROTROPH: e.g., a saprotrophic
protozoon. (Hence adj. saprozoic cf. SAPROTROPHIC.)
saquinavir See ANTIRETROVIRAL AGENTS.
saramycetin A polypeptide antifungal antibiotic produced by
Streptomyces saraceticus; it has been used e.g. against aspergillosis, blastomycosis and histoplasmosis.
Sarcina
A genus of Gram-positive, asporogenous, anaerobic
bacteria which occur e.g. in the gut in man and other animals. Cells: non-motile cocci (ca. 23 m diam.) which typically occur in cubical packets. The type species, S. ventriculi,
commonly has a CELLULOSE microcapsule. Metabolism is fermentative; the main products of glucose fermentation are acetic
acid and ethanol (in S. ventriculi ) or butyric and acetic acids (in
S. maxima). GC%: ca. 2931.
sarcina sickness See BEER SPOILAGE.
sarciniform (sarcinaeform) Arranged in PACKETS.
sarcinoid Refers to an alga in which the cells are more or less
SARCINIFORM. (See e.g. FRIEDMANNIA and PSEUDOTREBOUXIA.)
Sarcinosporon A genus of imperfect, non-fermentative fungi in
which both budding yeast cells and septate hyphae are formed;
blastospores develop from the mycelium, and septation in
different planes in the blastospores and hyphal cells results in the
formation of sarciniform clusters of cells. Asexual endospores
are formed. One species: S. inkin, isolated from a human skin
lesion. [Book ref. 100, pp. 906908.]
sarcocyst See SARCOCYSTIS.
Sarcocystis A genus of coccidian protozoa (suborder EIMERIORINA) which are obligately heteroxenous parasites in a range of
animals, including man (see SARCOSPORIDIOSIS). The vegetative
cells resemble those of TOXOPLASMA. In the intermediate host,
ingestion of oocysts or sporocysts is followed by schizogony in
internal organs, and merozoites later localize in muscle tissues;
a merozoite becomes rounded to form a metrocyte which, by
repeated division, gives rise to an immature sarcocyst: a collection of slowly-dividing metrocytes bounded by a cyst wall. Over
a period of ca. 2 months the contents of the sarcocyst change
from metrocytes only to a mixture of metrocytes and merozoites,
and finally (in the mature sarcocyst) to merozoites only. Ingestion of sarcocyst-containing flesh by the final host is followed
by sexual reproduction (only) in intestinal tissues: gametogony
is followed by ENDOSPORULATION, resulting in disporic, tetrazoic
oocysts, or free sporocysts, which are shed in faeces; the oocysts
lack a MICROPYLE, and the sporocysts lack a STIEDA BODY. (cf.
FRENKELIA.) [Taxonomy of Sarcocystis: J. Parasitol. (1986) 72
372382.]
sarcocystosis Syn. SARCOSPORIDIOSIS.
Sarcodina A subphylum of protozoa (phylum SARCOMASTIGOPHORA) in which the vegetative cells form one or more
pseudopodia (see PSEUDOPODIUM) or are motile by cytoplasmic
flow without the formation of discrete pseudopodia. Flagella are
formed only in temporary stages of certain species. In many
sarcodines the cytoplasm is more or less clearly differentiated
into an inner, typically granular, endoplasm (= granuloplasm
or plasmasol ) and a surrounding, typically hyaline layer (ectoplasm, hyaloplasm, plasmagel ) immediately beneath the plasmalemma. Sarcodine morphology ranges from the simple, naked,
amoeboid cell of e.g. Amoeba spp to relatively complex forms
sarcoidosis
with external tests (e.g. foraminifera) or internal skeletal structures (e.g. heliozoa, radiolaria). CYSTS are commonly formed.
Asexual reproduction occurs by fission; sexual processes occur
in some species. Sarcodines are commonly solitary, free-living
organisms in aquatic habitats, soil, etc; some are parasitic. There
are two superclasses: ACTINOPODA and RHIZOPODA.
sarcoidosis A chronic, granulomatous human disease which
resembles disseminated tuberculosis, with lesions (rarely
necrotic) in e.g. liver, lungs and spleen; other sites, including
skin, salivary glands and eyes may also be affected. The disease
is apparently self-limiting in the majority of cases.
Cause: unknown; Propionibacterium may be a better candidate than Mycobacterium [JCM (2002) 40 198204].
sarcoma A malignant tumour derived from connective tissue
e.g. bone (osteosarcoma), cartilage (chondrosarcoma), muscle
(rhabdomyosarcoma, = rhabdosarcoma), fat cells (liposarcoma),
lymphoid tissue (lymphosarcoma), etc. (cf. FIBROSARCOMA and
FIBROMA.) Sarcomas may be induced by infection with certain
viruses: see e.g. KAPOSIS SARCOMA, MURINE SARCOMA VIRUSES,
ROUS SARCOMA VIRUS, SIMIAN SARCOMA VIRUS.
Sarcomastigophora A phylum of PROTOZOA [JP (1980) 27
3758] which have flagella or pseudopodia or both; cells typically have a single type of nucleus. Subphyla: MASTIGOPHORA,
OPALINATA and SARCODINA.
sarcomatrix See RADIOLARIA.
sarconeme A MICRONEME in Sarcocystis.
Sarcoscypha See PEZIZALES.
sarcosine See SARKOSYL.
sarcosporidiosis Any disease of man and other animals e.g.
cattle, pigs, sheep caused by species of SARCOCYSTIS. In cattle and sheep the experimentally-induced disease can involve
lesions in a wide range of tissues and can lead to abortion (cf.
DALMENY DISEASE). In man the disease typically involves parasitization of the muscles, but experimentally-induced induced
disease, involving ingestion of meat infected with S. hominis,
leads to abdominal pain, diarrhoea, and the excretion of sporocysts. [AP (1982) 20 352396.]
sarcotoxins Antibacterial proteins produced in the haemolymph
of larvae of the flesh fly (Sarcophaga peregrinia) either on
exposure to bacteria or following mechanical injury; sarcotoxin I appears to affect cytoplasmic membrane functions in
Escherichia coli. [Sarcotoxin II: Biochem. (1987) 26 226230.]
(cf. CECROPINS.)
Sargassum See PHAEOPHYTA.
Sarkosyl An anionic detergent: N-lauroylsarcosine. (Sarcosine =
N-methylaminoacetic acid.)
SARS Severe acute respiratory syndrome: a sometimes-fatal
coronavirus infection [Lancet (2003) 362 263270; EID (2004)
10 (whole issue) 167387].
Sartorya A genus of fungi (order EUROTIALES) which include the
teleomorph of Aspergillus fumigatus.
satellite The posterior gregarine in SYZYGY. (cf. PRIMITE.)
satellite colonies See SATELLITE PHENOMENON.
satellite lesions Lesions remote from the original site of infection.
satellite phenomenon (satellitism) The phenomenon in which
certain growth-factor-requiring organisms can grow on a medium which lacks the required growth factor but which is supporting the growth of another (feeder) organism which can
supply the required growth factor a manifestation of SYNTROPHISM. For example, to determine the V factor requirement
of a Haemophilus strain, blood agar (in which V FACTOR is
unavailable) is inoculated with the Haemophilus strain, and the
Schiffs reagent
scarlet fever (scarlatina) An acute infectious human disease
which affects mainly children; it is caused by erythrogenic toxinproducing strains of Streptococcus pyogenes. Transmission may
occur by direct contact, by droplet infection, or via contaminated milk etc; infection usually occurs via nose or mouth,
occasionally via wounds or via the birth canal (puerperal scarlet
fever). Incubation period: 25 days. Symptoms: e.g. sore throat,
fever, swelling of the cervical lymph nodes, and a characteristic
bright-red punctate rash on the body followed by desquamation. The tongue often develops a greyish coating through which
the swollen red papillae can be seen (strawberry tongue). The
disease ranges from mild to severe or occasionally fatal. Complications: e.g. RHEUMATIC FEVER. Chemotherapy: e.g. penicillins,
erythromycin. (See also DICK TEST; SCHULZCHARLTON TEST.)
Non-streptococcal scarlatiniform rash (in which e.g. strawberry tongue does not occur) is caused e.g. by staphylococci.
SCAT SHEEP CELL AGGLUTINATION TEST.
Scatchard plot A graph which can be used to analyse molecular
interactions in a mixed population of molecules in which
molecules of different types bind reversibly to one another.
In serology, for example, a Scatchard plot can indicate (i) the
association constant (= AFFINITY) of antigenantibody binding
(given by the slope of the curve); (ii) the nature of the antibody
population: MONOCLONAL ANTIBODIES give a straight-line plot,
while POLYCLONAL ANTISERUM gives a curved plot; and (iii) the
number of binding sites per molecule.
Scedosporium See PSEUDALLESCHERIA and HYPHOMYCETES.
Scenedesmus
A genus of non-motile, coenobial green algae
(division CHLOROPHYTA) which occur often abundantly in a
wide range of freshwater habitats. The coenobia each consist
of 2, 4, 8, or occasionally 16 elongate or fusiform cells in a
palisade arrangement (i.e., side-by-side). In some species the
two outermost cells bear a spine or tuft of bristles at each corner
of the free side of the cell; however, morphology may vary
considerably according to environmental conditions. Each cell
contains one nucleus and one chloroplast which usually has a
single conspicuous pyrenoid. Asexual reproduction occurs by the
formation of a complete daughter coenobium within each cell of
a parent coenobium; the daughter coenobia are released often
explosively by rupture of the parent cell wall. Biflagellate
zoospores may also be formed, at least in some species. Sexual
reproduction involves the formation of biflagellate isogametes.
SchaefferFulton stain See ENDOSPORE STAINS.
Schardinger dextrins (cycloamyloses or cyclodextrins) Cyclic
DEXTRINS formed from starch or glycogen by an extracellular
enzyme, cyclodextrin glucosyltransferase, from Bacillus macerans (a similar enzyme is produced e.g. by B. megaterium);
a-, b- and g-cyclodextrins contain 6, 7 and 8 (1 4)-a-linked
D-glucose residues, respectively.
Schaudinns fluid A FIXATIVE: mercuric chloride (100 ml saturated, aqueous) and 95% ethanol (50 ml) supplemented immediately before use with glacial acetic acid (1.5 ml).
scheduled diseases NOTIFIABLE DISEASES of animals.
Schellackia See EIMERIORINA.
Schick test A test which determines a persons susceptibility to
DIPHTHERIA. Diphtheria toxin is injected intradermally into one
arm; as a control, inactivated toxin is injected into the other arm.
A positive test (person susceptible) is indicated, after several
days, by an inflammatory response at the site of injection of the
potent toxin. No reaction (negative test) indicates the presence
of antitoxin and hence resistance to the disease.
Schiffs reagent Basic FUCHSIN decolorized with sulphurous acid;
it reacts with aldehydes to give a red-purple colour. (See FEULGEN
REACTION and PAS REACTION.)
689
Schizoblastosporion
in which there is a large kinetoplast situated close to the pointed
posterior end of the cell, and a free flagellum; intracellular
amastigote and epimastigote forms occur in pseudocysts. In the
vector, epimastigotes, sphaeromastigotes and metacyclic forms
occur in the gut and rectum. [Cell biology of T. cruzi: Int. Rev.
Cytol. (1984) 86 197283.] T. (S.) c. cruzi can be cultured
in e.g. NNN MEDIUM. [A minimal medium for the cultivation
of infective T. cruzi epimastigotes: JGM (1983) 129 285291;
improved method for purification of metacyclics from the insect
vector Triatoma infestans: JP (1986) 33 132134.]
schlepper (immunol.) Any substance which, by combining with
a second substance, promotes the immunogenicity of the latter.
schlieren system An optical system for measuring a refractive
index gradient.
Schmutzdecke
The film or layer of microorganisms which
develops e.g. in a slow sand filter (see WATER SUPPLIES); it usually
contains algae, bacteria and protozoa.
Schuffners
dots In erythrocytes infected with Plasmodium vivax
Scuticociliatida
PARATYPHOID FEVER (2)), but also a symptom e.g. of certain
mycotoxicoses and of secondary copper deficiency syndromes
(e.g. peat scours, scouring disease, teart) in ruminants. (See also
CALF SCOURS; TRANSMISSIBLE GASTROENTERITIS; WINTER DYSENTERY.)
SCP SINGLE-CELL PROTEIN.
scrapie A TRANSMISSIBLE SPONGIFORM ENCEPHALOPATHY (q.v.)
which, in nature, affects sheep and goats. After an incubation
period of months or years the infected animal exhibits neurological symptoms e.g. evidence of intense itching, incoordination and trembling followed by emaciation and (after weeks
or months) death. Histopathology in the central nervous system: e.g. vacuolation, gliosis and astrocytosis. No inflammatory
response is elicited at any stage, interferons are not induced, and
there is no specific immune response. Different breeds of sheep
differ markedly in their susceptibility to scrapie.
The causal agent is a PRION designated PrPsc . It can be
transmitted experimentally e.g. to mice and hamsters in which
animals the disease follows a much shorter course and may
involve different symptoms (for example, scrapie-infected mice
do not scratch). PrPsc is initially demonstrable in the spleen
and lymphoid tissues; eventually it reaches maximum titres
in the brain. Abnormal, amyloid-like fibrillar structures can
be seen in synaptosomal and spleen preparations of infected
mice; these scrapie-associated fibrils (SAFs) contain a protein
subunit formerly designated PrP 2730 (because its MWt was
apparently 2700030000). SAFs appear to be closely associated
with infectivity.
screening test (1) Any test used to detect the presence of a given
agent (e.g. a specific antibody or microorganism) in each of
a large number of specimens; such tests are typically simple
and inexpensive but are usually not completely specific for
the antibody or microorganism. A certain proportion of falsepositive results may be tolerated as a positive screening test may
be followed up by other tests which are more specific. (2) Any
test which enables a given (unknown) organism to be assigned
to one of a possible range of taxa.
scRNA Small cytoplasmic RNA. scRNAs occur in the cytoplasm
of eukaryotic cells in the form of ribonucleoprotein particles
(scRNPs or scyrps), including PROSOMES. (cf. SNRNA.)
scrofula Cervical lymphadenitis caused by Mycobacterium scrofulaceum or by other members of the MAC.
scrub typhus (tsutsugamushi disease) An acute, systemic human
disease caused by Rickettsia tsutsugamushi (= R. orientalis) and
transmitted by the bite of the larval stage of a trombiculid mite;
rodents are a reservoir of infection. The disease occurs in Asia,
Australia, and the Pacific area. Incubation period: 13 weeks. A
primary lesion (an ESCHAR) often develops at the location of the
bite; subsequent symptoms resemble those of epidemic typhus
(see TYPHUS FEVERS). Lab. diagnosis: e.g. the WEILFELIX TEST.
Chemotherapy: tetracyclines, chloramphenicol.
SCSR See CLOVER ROT.
Scutellinia
A genus of fungi (order PEZIZALES) which form
apothecia bearing dark, pointed setae. S. scutellata (common
on rotting wood) forms brick-red apothecia typically several
millimetres across.
scutica In members of the SCUTICOCILIATIDA: a transient, hooklike structure, consisting of a number of (generally non-ciliated)
kinetosomes, formed during STOMATOGENESIS.
Scuticociliatida An order of protozoa (subclass HYMENOSTOMATIA) in which somatic ciliature is uniform to sparse (sometimes
involving distinctive caudal ciliature), and in which the buccal
ciliature often includes a large, protruding and conspicuous PARORAL MEMBRANE; STOMATOGENESIS is buccokinetal and involves
scutulum
and the sequence 5 -GTTGAC-3 is used as a terminal tag in
both primers (S1 and S2).
During amplification of the target in SDA, all strand synthesis is carried out in a reaction mixture that contains a
chemically modified form of deoxyadenosine triphosphate: athiophosphoryl dATP (dATPaS). Hence, when a complementary strand is synthesized on the HincII site of a primer, the
sequence (3 . . . CAACTG . . . 5 ) contains two of the modified
nucleotides (AA) adjacent to the cleavage site; this strand is
resistant to cleavage by HincII i.e. the double-stranded HincII
site contains one cleavable sequence (in the primer) and one
non-cleavable sequence (in the newly synthesized, complementary strand). Such a hemi-modified or hemiphosphorothioate
HincII site can be nicked between T and G in the primer
strand. When such a nick is made, the polymerase can extend
the 3 end and displace the strand downstream of the nick site.
Importantly, note that the strand formed by extension from
the nick site (5 -GTT ) will incorporate a modified
nucleotide at the A position of GAC; despite this, the HincII
site in the newly synthesized strand 5 -GTTGAC.....3 is nickable i.e. incorporation of a single modified nucleotide in GAC
does not affect nickability (unlike the incorporation of two modified nucleotides in the sequence 3 . . . CAACTG . . . 5 in the
complementary strand).
In practical terms the method is uncomplicated. Essentially,
sample dsDNA is heat-denatured in a reaction mixture containing all components except the polymerase and restriction
endonuclease; the mixture is cooled to an appropriate temperature, the enzymes are added, and incubation is continued for the
required period.
SDA-based diagnostic procedures are being developed by the
Becton Dickinson organization. The BDProbe Tec system has
been tested for its ability to detect Mycobacterium tuberculosis
in respiratory specimens [JCM (1999) 37 137140], and a more
recent system, BDProbe Tec ET, has been evaluated for the
detection of Chlamydia trachomatis and Neisseria gonorrhoeae
[CC (1999) 45 777784].
[SDA, NASBA, TMA in clinical microbiology: Book ref. 221,
pp 126151.]
SDS Sodium dodecyl (= lauryl) sulphate.
SDS-PAGE (Laemmli electrophoresis [Nature (1970) 227 680
685]) Sodium dodecyl sulphate polyacrylamide gel electrophoresis: a specialized form of ELECTROPHORESIS used e.g. for
determining the molecular weight of a protein, or for separating
mixtures of proteins.
Molecular weight determination by SDS-PAGE. At concentrations > ca. 104 to 103 M, sodium dodecyl sulphate (SDS;
CH3 (CH2 )11 OSO3 Na) binds cooperatively to proteins and denatures them, forming long rod-like SDS-polypeptide complexes;
virtually all proteins bind a similar amount of SDS per unit
weight of protein. Each SDS molecule binds via its hydrophobic end, and the coating of SDS molecules effectively masks
the charges on the polypeptide. Since the length of an SDSpolypeptide complex is roughly proportional to the molecular
weight of the polypeptide, the electrophoretic mobility of such
a complex will give an approximate indication of the molecular weight of the polypeptide. Thus, if the SDS complex of an
unknown protein is subjected to PAGE together with the SDS
complexes of reference proteins (of known molecular weights),
the molecular weight of the unknown protein can be calculated
by comparing the electrophoretic mobilities.
Some proteins (e.g. pepsin, many viral capsid proteins)
form SDS complexes only if they are heated in the presence
the appearance of a SCUTICA. Cyst formation is common. Genera include e.g. Ancistrum, Boveria, CYCLIDIUM, Loxocephalus,
Parauronema, Philaster, Pleuronema, and Uronema.
scutulum See FAVUS.
ScV Saccharomyces cerevisiae virus (see MYCOVIRUS).
scyllitol See INOSITOL.
Scyphidia See PERITRICHIA.
scyphus (lichenol.) See PODETIUM.
scyrps See SCRNA.
Scytonema
A genus of filamentous CYANOBACTERIA (section
IV) in which the mature trichomes are uniform in width (cf.
CALOTHRIX) and are composed of disc-shaped, isodiametric or
cylindrical vegetative cells; young trichomes from hormogonia
each have a heterocyst at only one end. GC%: ca. 44.
In nature, trichomes are heavily ensheathed and exhibit
frequent FALSE BRANCHING. A distinction is often made between
Tolypothrix (false branches occur singly) and Scytonema (false
branches occur in pairs); however, since false branching is
variable in culture, these two genera are generally considered as
one, Scytonema [Book ref. 45, p. 254]. (See also STROMATOLITE.)
Scytosiphon See PHAEOPHYTA.
SD sequence (SD region) ShineDalgarno sequence: see PROTEIN SYNTHESIS.
SDA Strand displacement amplification: a method for copying
(amplifying) a given sequence of nucleotides in DNA. Like
NASBA (but unlike LCR or PCR), SDA is carried out isothermally;
originally the operating temperature was 40 C but, owing
to suboptimal specificity, it was later raised to 50 C (=
thermophilic SDA; tSDA).
SDA is considerably more complex than other nucleic-acidamplification procedures. It has two distinctive features: (i) the
use of a DNA polymerase which can displace an existing strand
of DNA by using the complementary strand as a template,
and (ii) the use of a RESTRICTION ENDONUCLEASE for repeatedly
nicking a modified cutting site in a mechanism for regenerating
templates.
Only certain types of DNA polymerase are able to carry out
strand displacement one of which is the exonuclease-deficient
form of the KLENOW FRAGMENT. As illustrated in the figure, the
strand-displacing activity of a polymerase can be manifested
in two ways. In one mode, a so-called bumper primer binds
upstream of the strand to be displaced; extension of the 3 end
of the bumper primer by a (strand-displacing) DNA polymerase
displaces the strand downstream. (In SDA, displacement of the
5 end of the strand begins while the 3 end is still being
synthesized.) The second mode of strand displacement occurs
at a NICK site; here, the polymerase extends the 3 end of the
nick and, in so doing, displaces the downstream region of the
same strand. (In effect, the 3 end at the nick site functions as a
primer.)
The restriction endonuclease used in SDA is HincII; it has
the (generalized) recognition site:
5 .....GTPy/PuAC.....3
3 .....CAPu/PyTG.....5
(Py = a pyrimidine, Pu = a purine). The oblique (/) indicates
the cleavage site in each strand; thus, HincII normally makes a
blunt-ended cut across both strands.
The specific HincII recognition site used in SDA is:
5 .....GTT/GAC.....3
3 .....CAA/CTG.....5
692
B1
S1
amplicon
(a)
( antisense )
S1
(b)
( sense )
( sense )
S1
(c)
S2
(d)
(e)
B2
5
3
3
5
(f)
(g)
(h)
To amplification phase
SDA (strand displacement amplification) I: the target-generation phase (diagrammatic). The target DNA is denatured by heat to the
single-stranded form prior to SDA.
(a) The antisense (3 -to-5 ) strand of the target duplex showing the amplicon delimited by two short, vertical bars. (For clarity, and economy
of space, only one strand of the amplicon is considered; corresponding events occur on the complementary strand.) A primer (S1) has bound
at the 3 end of the amplicon; the 5 end of this primer is tagged with (one strand of) the HincII recognition sequence: (5 -GTTGAC-3 ) (
). A
bumper primer (B1, see entry) has bound upstream of primer S1. Extension of S1 will produce a sense strand on the antisense template, and
this strand will be displaced when B1 is extended; the displaced sense strand is shown at (b).
(c) Primer S2 has bound at the 3 end of the amplicon on the sense strand; like S1, its 5 end is tagged with the recognition sequence of
HincII. The bumper primer B2 has bound upstream of S2. Extension of S2 produces an antisense amplicon which is tagged at both ends by a
HincII recognition sequence; this strand, which is displaced by the extension of B2, is shown at (d). Notice that the 3 HincII sequence in this
strand, having been synthesized with dATPaS, is modified as indicated by (
); this sequence is not susceptible to HincII.
(d) Primer S1 (not shown) binds at the 3 end of this strand, the HincII sequence in S1 hybridizing with the modified sequence in the strand.
Extension of S1 forms the double-stranded amplicon at (e). Each end of this amplicon consists of a hemi-modified recognition site for HincII; a
hemi-modified site can be nicked in the non-modified strand (arrowhead). Nicking of the upper strand at (e) is followed by extension of the 3
end of the nick this displacing the strand downstream of the nick site; this displaced strand is shown at (f).
(g) Primer S2 binds to the displaced strand. Extension of S2 forms the product at (h).
(h) This double-stranded product feeds into the amplification phase (see part II of figure).
693
(Par t I (a))
(a)
3
5
(b)
3
5
(antisense)
S1
(c)
5
AUGMENTED BY PRODUCT
(d)
(e)
(sense)
(sense)
(f)
S2
(g)
3
5
694
secretory component
the stipe, the lamellae are characteristically convoluted, and the
spores are not forcibly discharged; the secotioid fruiting body
may be epigean or hypogean, the latter type closely resembling
the fruiting body of a typical gasteromycete. Secotioid fungi are
found in various taxa; they include e.g. certain members of the
Russulales. Secotium, formerly classified in the Agaricales, is
now included in the Gasteromycetes (Podaxales). [The secotioid
syndrome: Mycol. (1984) 76 18.]
Secotium See SECOTIOID FUNGI.
secretin Any one type of a family of proteins which oligomerize
to form pores in the OUTER MEMBRANE; in at least some cases
the multimeric pores are stabilized by a specific outer membrane
lipoprotein.
One example of a secretin is the PilQ protein of Neisseria
gonorrhoeae; this protein, which is involved in the formation
of type IV FIMBRIAE, forms an outer membrane pore that is
stabilized by the PilP protein. Another example is the usher
protein, PapC, involved in the formation of P fimbriae (type I
fimbriae); the corresponding structure is stabilized by the PapH
protein. The YscC protein of the Yersinia VIRULON is a further
example.
secretion (of a protein) The transmembrane translocation of a
protein, towards the cells exterior, with eventual release of the
protein to the external environment. (cf. EXPORT.)
secretion of proteins (by Gram-negative bacteria) See PROTEIN
SECRETION.
secretion sequence See ABC EXPORTER.
secreton In type II PROTEIN SECRETION systems: the complex of
proteins which, together, enable proteins to cross the OUTER
MEMBRANE, i.e. the terminal branch of the type II system; thus,
a protein may be translocated across the cytoplasmic membrane
in a sec-dependent manner and then secreted to the cells exterior
via the secreton.
The secreton is functionally analogous to the protein transport
system involved in the formation of certain fimbriae [EMBO
(2000) 19 22212228].
secretory ampulla Syn. AMPULLA sense 1 or 2.
secretory component (secretory piece) A glycoprotein (MWt ca.
60000) produced (as a membrane protein) in hepatocytes and in
epithelial cells of various mucosal surfaces in the body; it is
a component of sIgA (see IgA). Secretory component binds to
SDA (strand displacement amplification) II (continued) (c) Each antisense strand from (b) can bind primer S1. Extension of S1, and of the
(recessed) 3 end of the antisense strand, forms the product at (d). Extension of the 3 end of the antisense strand has formed a modified,
non-nickable HincII restriction sequence (
) because the three terminal nucleotides in this strand (3 -CAA-5 ) include two modified
nucleotides (dATPaS).
(d) This product has a nickable restriction site (arrowhead) derived from primer S1. Like the product at (a), it can undergo a cyclical process
of nicking, strand extension and regeneration, concurrently displacing copies of a single-stranded product; however, this single-stranded
product is a sense strand of the target sequence. The regenerated product and sense strand are shown at (e).
Recall that part I illustrates the events arising from DNA synthesis on the antisense strand of the target duplex. If events are followed on the
sense strand, the resulting product is identical to that shown here at (d).
(e) The single-stranded (sense) product shown here is able to bind primer S2.
(f) The single-stranded product from (e) has bound primer S2. DNA synthesis (i.e. extension from S2, and also from the recessed end of the
sense strand) then gives rise to the product seen at (g). (DNA synthesis at the 3 end of the sense strand forms a non-nickable restriction site
for the reason given under (c), above.)
(g) This product is equivalent to the one shown at (a).
Summarizing, two types of double-stranded product from the target-generation phase, derived from different strands of the target, undergo
cyclical nicking, strand synthesis and regeneration, concurrently displacing numerous copies of antisense and sense strands of the target
sequence. Antisense strands bind primer S1 and form the (double-stranded) product which yields sense strands; sense strands bind primer S2
and form the (double-stranded) product which yields antisense strands. Nickable HincII restriction sites are provided by the 5 -tags on S1 and
S2 primers (which are present in excess in the reaction mixture).
Parts I and II reproduced from Figures 5.3 and 5.4, pages 134137, in DNA Methods in Clinical Microbiology (ISBN 07923-6307-8), Paul
Singleton (2000), with kind permission from Kluwer Academic Publishers, Dordrecht, The Netherlands.
695
secretory IgA
selenite broth (selenite F broth) A MEDIUM used e.g. for the
ENRICHMENT of strains of Salmonella in samples of faeces; selenite inhibits many of the common enteric bacteria. The medium
consists of an aqueous solution of peptone (0.5%), lactose or
mannitol (0.4%), NaHSeO3 (0.4%), and either Na2 HPO4 (1.0%)
or a combination of Na2 HPO4 and NaH2 PO4 to give a final pH
of ca. 7.0. The medium should not be autoclaved, but may be
steamed for 30 min. Incubation of the inoculated medium should
not exceed ca. 1218 hours.
Selenococcidium See EIMERIORINA.
Selenomonas A genus of Gram-negative bacteria (family BACTEROIDACEAE) which occur e.g. in the RUMEN and in the human
gingival crevice. Cells: curved (crescent- or kidney-shaped) rods,
0.91.1 3.06.0 m, with a tuft of flagella arising from the
concave side of the cell. Substrates include sugars and, sometimes, amino acids and lactate; glucose fermentation yields propionic and acetic acids as major products together with e.g.
CO2 and/or lactate. GC%: ca. 5461. Type species: S. sputigena
(which does not ferment cellobiose, dulcitol or salicin, and which
occurs in the human mouth); other species: S. ruminantium
(which ferments cellobiose, dulcitol and salicin, and which
occurs in the rumen).
Selenophoma A genus of fungi of the COELOMYCETES.
self-cloning experiment A CLONING experiment in which the
DNA to be cloned is derived from the same strain or species
as that in which the recombinant DNA is to be replicated; a
recombination-deficient strain may be used to prevent recombination between the cloned DNA and the organisms genome.
self fertilization (protozool.) Syn. AUTOGAMY.
self purification The natural process in which organic material
(faeces etc) in rivers, streams etc undergoes MINERALIZATION,
and the resulting simple substances (e.g. nitrates) are made
available to photosynthetic and other organisms. Self purification
can occur only if the polluting load is not excessive. (See also
SAPROBITY SYSTEM.)
self-splicing introns See SPLIT GENE (b) and (c).
self tolerance (natural immunological tolerance) Unresponsiveness of the immune system to an individuals own (autologous)
antigens.
self-transmissible plasmid See CONJUGATIVE PLASMID.
selfing (ciliate protozool.) Syn. CYTOGAMY.
Seliberia A genus of Gram-negative, iron-accumulating, BUDDING BACTERIA which occur e.g. in soil; the organisms typically occur as radial clusters of rod-shaped cells. [Book ref. 45,
pp. 516519.]
Selysina See EIMERIORINA.
SEM See ELECTRON MICROSCOPY (b).
semiapochromatic objective Syn. FLUORITE OBJECTIVE.
semiconservative replication Replication of a double-stranded
nucleic acid such that each daughter duplex contains one parental
strand and one new strand. (See DNA REPLICATION.)
semipermissive cells (virol.) A cell population in which only
some of the cells are permissive for lytic infection by a given
virus. (cf. PERMISSIVE CELLS; see also CARRIER CULTURE.)
semipersistent transmission See NON-CIRCULATIVE TRANSMISSION.
semi-rough mutant See SMOOTHROUGH VARIATION.
semi-solid agar See AGAR and MEDIUM.
Semliki Forest virus (SFV) An ALPHAVIRUS which was first isolated from mosquitoes in Uganda. Its natural hosts and vectors
are unknown, but antibodies to the virus have been detected in
humans and wild primates in various parts of Africa, Malaya
and North Borneo. The virus is apparently non-pathogenic in
septum
must be treated, e.g. by aerobic biological oxidation or (when
permissible, and when underground water supplies would not
be contaminated) allowed to disperse in the soil below the
surface (subsurface irrigation). A septic tank can serve e.g.
150 houses. (cf. CESSPOOL; see also SEWAGE TREATMENT.)
septicaemia (septicemia; blood poisoning) A particular form of
BACTERAEMIA in which there are clinical symptoms (e.g. fever).
The term may also refer to the presence of Candida albicans or
other fungi in the bloodstream. (cf. VIRAEMIA.)
(See also SEPSIS and SIRS.)
septicemia Syn. SEPTICAEMIA.
septicolysin See THIOL-ACTIVATED CYTOLYSINS.
Septobasidiales An order of fungi (subclass PHRAGMOBASIDIOMYCETIDAE) which form non-gelatinous fruiting bodies; they
include parasites of scale insects (insects of the superfamily
Coccoidea). Genera: Septobasidium and Uredinella.
Septobasidium See SEPTOBASIDIALES.
septoria A plant disease caused by a species of Septoria: see e.g.
GLUME BLOTCH and HALO SPOT.
Septoria
A genus of fungi (order SPHAEROPSIDALES) which
include many plant pathogens e.g. S. apiicola, the causal agent
of late blight (leaf spot) of celery. (See also e.g. GLUME BLOTCH
and HALO SPOT.) Conidia are filiform and typically multiseptate
and colourless; they are formed in dark, ostiolate pycnidia
immersed in the substratum.
septum (cross-wall) (a) (bacteriol.) A partition which (i) divides
a parent cell into daughter cells during BINARY FISSION, (ii) occurs
between adjacent cells in a filament (see e.g. ACTINOMYCETALES),
and (iii) separates a developing ENDOSPORE from the rest of the
mother cell.
Septum formation is an essential phase in the CELL CYCLE (q.v.
for details of septum formation in bacteria).
During sporulation in Bacillus subtilis, one of the early stages
is the formation of an asymmetric septum, i.e. one which (unlike
that formed during cell division) develops near one pole of the
cell. Initially, an FtsZ ring (see CELL CYCLE) forms at the midcell position but then become helical and finally forms an FtsZ
ring at both polar sites; septation occurs at only one site [Science
(2002) 298 19421946].
(b) (mycol.) A partition, one or more of which divides certain
fungal structures (hyphae, spores etc.) into cells; septa are also
formed in fission yeasts (e.g. Schizosaccharomyces) during cell
division.
A primary septum is one formed in association with nuclear
division, i.e. one serving to separate daughter cells. An adventitious septum develops independently of nuclear division.
Septate hyphae are characteristic of the higher fungi, but septa
are also formed in certain lower fungi although often only in
ageing hyphae and/or in order to delimit reproductive structures
(such as sporangia).
Septate (multicellular) spores are formed by various fungi (e.g.
macroconidia in Fusarium).
In general, true septa (eusepta) have essentially the same
composition as the hyphal CELL WALL, but certain fungal structures (e.g. the mycelium of some of the more complex chytridiomycetes, and the conidia in certain hyphomycetes) have
septum-like pseudosepta (= distosepta) whose composition is
distinct from that of the cell wall.
Hyphal septa appear always to be formed by centripetal
growth from annular rims which develop on the inner surface of
the hyphal wall. In some cases growth of the septum continues
inwards until a complete plate is formed. In other cases, growth
stops before the septum is complete, so that a small pore (ca.
man. When injected into mice, SFV can cause an acute, lethal
encephalitis; virulent strains appear to damage neurones (or particular neurone subsets) directly, while other strains infect oligodendrocytes and cause demyelination apparently by triggering
an autoimmune response [JGV (1985) 66 23652373; review:
JGV (1985) 66 395408]. SFV can be transmitted transplacentally in mice, causing e.g. abortion or malformation of infected
fetuses. (See TOGAVIRIDAE for replication cycle etc.)
Semple vaccine An anti-RABIES vaccine consisting of a phenolinactivated preparation of rabbit-fixed rabies virus (i.e. rabies
virus passaged in rabbit brain).
sen gene See EIEC.
Sendai virus See PARAMYXOVIRUS.
senior synonym See SYNONYM.
sennetsu rickettsiosis See EHRLICHIA.
sens. lat. SENSU LATO (q.v.).
sense codon A codon which specifies an amino acid: see GENETIC
CODE.
sense strand (of DNA) See CODING STRAND.
sensitin Any preparation (e.g. an extract of a given microorganism, as in brucellin, coccidioidin etc) which can act as an
ALLERGEN; sensitins are used in SKIN TESTS.
sensitivity agar Any of various standardized, solid, agar-based
media used for carrying out ANTIBIOTIC-sensitivity tests.
sensitization (immunol.) (1) (of a person or animal) The initial
exposure of an individual to an allergen such that a manifestation
of HYPERSENSITIVITY occurs on subsequent exposure(s) of the
individual to that allergen. (2) (of persons, animals or cells)
The process of priming (see PRIMED). (3) The combination
of cell-surface antigens with their homologous antibodies (see
e.g. HAEMOLYTIC SYSTEM). (4) The coating of erythrocytes with
soluble antigens (see BOYDEN PROCEDURE). (5) Any procedure of
the type in which certain strains of staphylococci are coated
(sensitized) with unrelated antibodies (see PROTEIN A) for use
in a PASSIVE AGGLUTINATION TEST for the homologous antigen.
(6) The combination of cells with cytophilic antibodies (see e.g.
REAGINIC ANTIBODIES).
sensu lato (s.l.; sens. lat.) Of a term or name: (1) used in a broad
or more inclusive sense, or (2) used with a meaning other than
the original meaning.
sensu stricto (s.s.; s. str.) Of a term or name: (1) used with a precise or narrow meaning, or (2) used with the original meaning.
Seoul virus See HANTAVIRUS.
sepB gene See PATHOGENICITY ISLAND.
Sephadex See DEXTRANS and GEL FILTRATION.
Sepik virus See FLAVIVIRIDAE.
sepsis (med., vet.) (1) The state in which pathogen(s) are present
in particular tissue(s). (cf. ASEPSIS; SEPTICAEMIA.) (2) The symptoms associated with microbial infection of tissues. (See also
SIRS.)
septa Plural of SEPTUM.
septal pore cap See DOLIPORE SEPTUM.
septate Having one or more septa.
septic (1) (med., vet.) Refers to SEPSIS (generally sense 2).
(2) Refers to the presence or activities of microorganisms
involved in putrefaction or decay (see e.g. SEPTIC TANK).
septic diphtheria See DIPHTHERIA.
septic shock Syn. ENDOTOXIC SHOCK.
septic tank A ventilated tank into which domestic sewage flows
and within which the sewage undergoes primary purification
(settlement of suspended solids) and some degree of ANAEROBIC
DIGESTION; solids (sludge and scum) are periodically removed
for disposal. The highly polluting supernatant overflows and
697
being linked to the conversion of glyoxylate to glycine. The reaction sequence continues thus: hydroxypyruvate glycerate
2-phosphoglycerate, the latter either being converted to 3phosphoglycerate (phosphoglycerate mutase, EC 2.7.5.3) and
assimilated into biomass, or converted to phosphoenolpyruvate
(PEP). CO2 enters the cycle at this point: with PEP (PEP carboxylase, EC 4.1.1.31) it forms oxaloacetate. The cycle continues oxaloacetate malate malyl-CoA, the latter being split
(by a lyase, EC 4.1.3.24) to glyoxylate (used to regenerate
glycine see above) and acetyl-CoA. Acetyl-CoA with oxaloacetate (citrate synthase) initiates a subsidiary cycle, first forming
citrate and then isocitrate which is split (isocitrate lyase, EC
4.1.3.1) to glyoxylate and succinate, the latter being converted,
in several steps, to oxaloacetate which re-enters the subsidiary
cycle [see Appendix II(b)]; as before, glyoxylate is used to
regenerate glycine.
The pathway described above is referred to as the icl or
icl+ (isocitrate lyase) serine pathway. Some organisms which
use the serine pathway (e.g. Pseudomonas AM1) contain
neither malate thiokinase (and hence cannot form malyl-CoA)
nor isocitrate lyase (and hence cannot regenerate glyoxylate in
the subsidiary cycle); the pathway in these organisms is called
the icl serine pathway. The way in which acetyl-CoA is used
to regenerate glyoxylate (and glycine) in the icl serine pathway
is not yet understood; in the proposed homo-isocitrate pathway
acetyl-CoA condenses with 2-oxoglutarate to form homocitrate
and then homoisocitrate which is cleaved to glyoxylate and
glutarate the latter being used to regenerate 2-oxoglutarate.
serine proteases See PROTEASES and type II systems in PROTEIN
SECRETION.
seroconversion The development of antibodies in response to
exposure to antigen.
seroconversion illness See AIDS.
serodiagnosis Diagnosis based on serological tests.
serofactor 1 See YERSINIA (Y. pestis).
serofast Refers to a patient whose serum (sampled at intervals
of time) consistently gives positive results in a given serological
test.
serological tests for syphilis Syn. STANDARD TESTS FOR SYPHILIS.
serological typing See TYPING.
serology The study of in vitro reactions involving one or more
of the constituents of SERUM (e.g. a particular type of ANTIBODY, or a component of COMPLEMENT) or of PLASMA (see e.g.
clumping factor in COAGULASE); serology is used e.g. in medical diagnostic procedures to detect and/or quantify particular
antigens or antibodies. See e.g. HAEMAGGLUTINATION-INHIBITION
TEST, IMMUNOASSAY, WIDAL TEST.
serotonin 5-Hydroxytryptamine: a base (derived from tryptophan) with physiological activity similar to that of HISTAMINE; it
occurs e.g. in the platelets of many species, and is also found
e.g. in the MAST CELLS and basophils of some species.
(See also ENTEROCHROMAFFIN CELLS.)
serotype (serological type; serovar) A serologically (antigenically) distinct VARIETY (usually) within a bacterial species.
serotyping A method of TYPING in which strains are distinguished
on the basis of differences in their surface ANTIGENS (e.g. cell
wall, flagellar and/or capsular antigens). Essentially, each strain
to be typed is tested with a variety of antibodies (different
antibodies being specific for antigens on different strains of
the organism). If the cells of an unknown (i.e. untyped) strain
bind a particular antibody (indicated in vitro by agglutination or
precipitation of the cells), the unknown strain is placed in the
same category (type) as the strain homologous to that antibody.
698
DREYERS TUBE)
699
severin
dispose of, the grosser debris; the screened sewage may then be
passed through a comminutor (a rotary shredding device which
breaks up the smaller solids). The screened, comminuted sewage
effluent then passes slowly through a sedimentation (settlement)
tank in which some particulate matter settles out (and is removed
as sludge). Sedimentation is sometimes assisted by the addition
of alum as the effluent enters the sedimentation tank.
Secondary treatment is designed to reduce the BOD of the
primary effluent to acceptable levels by microbial oxidation of
the dissolved organic content. This is usually achieved by one of
three types of (aerobic) process: the trickle filter, the activated
sludge process and the (more recent) biological aerated filter
(BAF); these processes are considered below.
The trickle filter (biological filter, percolating filter ) consists
of a bed of crushed rock, ca. 2 m deep, over which the primary
sewage effluent is sprayed. The bed of rock may be enclosed
within a circular wall, the sewage being sprayed through holes
in the arms of a rotary sprinkler; with a rectangular bed of rock,
sewage is sprayed from a distributor arm moving backwards and
forwards. The rock surface bears a film of microorganisms for
example, the bacterium Zoogloea ramigera and species of
ciliate protozoa (e.g. Carchesium, Chilodonella, Opercularia
and Vorticella). (Also commonly present are e.g. rotifers,
crustaceans, insects and arachnids.)
Percolating slowly through the crushed rock, the sewage
makes close contact with surfaces that bear the biofilm. The
sprayed sewage carries with it dissolved oxygen, so that some
of the dissolved organic matter can be oxidized by organisms
in the sewage and by those in the biofilm; moreover, some
dissolved organic carbon is assimilated, as biomass, by these
organisms. The system is not intended to act as a mechanical
sieve but rather to permit close contact between the biofilm
and sewage under aerobic conditions; this reduces the level of
dissolved organic matter. Moreover, large numbers of sewage
bacteria are ingested by protozoans in the biofilm.
Effluent leaving the bed usually contains small particles of
biofilm washed from the rock; these particles may be allowed
to settle in a humus tank before the supernatant is discharged as
the final effluent. The final effluent has a much lower BOD so
that, if discharged to a river etc., it will take less oxygen from
the water.
The activated sludge process is another form of aerobic secondary treatment. Effluent from the primary treatment stage
enters a vessel containing activated sludge a mass of organisms consisting mainly of bacteria (e.g. species of Acinetobacter
and Alcaligenes, Sphaerotilus natans and Zoogloea ramigera)
and protozoa; the latter include ciliates (e.g. Aspidisca, Carchesium, Opercularia, Trachelophyllum, Vorticella), flagellates, and
the testate amoebae Cochliopodium and Euglypha amoebae
often being found in large numbers and sometimes forming
the major component of the biomass. Other organisms present
include fungi, rotifers and nematodes. Effluent and sludge are
vigorously agitated and aerated for e.g. 612 hours so that much
of the soluble organic matter in the effluent is oxidized, or assimilated, by the biomass; the BOD is thus greatly reduced, and large
numbers of sewage bacteria are ingested by protozoa. The treated
effluent is then left in a sludge-settling tank. Good-quality final
effluent depends on efficient flocculation (= aggregation) of the
organisms, this facilitating clarification of the effluent by sedimentation. Flocculation is encouraged by cell-surface hydrophobicity which promotes (i) adherence of cells to flocs, and (ii)
penetration of the flocs by cells via channels/pores within the
shaded matrix
by using a cycle of alternating anaerobic and aerobic treatments. Anaerobically, some organisms increase in biomass but
release phosphorus; aerobically, the (increased) biomass assimilates phosphorus and is subsequently separated and disposed
of. The bacterium Acinetobacter calcoaceticus is reported to
accumulate phosphate (up to 10% dry weight), >50% as
POLYPHOSPHATE. [Biological phosphorus removal: MS (1984) 1
149152. Identification of polyphosphate-accumulating bacteria
for biological phosphorus removal in activated sludge plants:
AEM (2000) 66 11751182.]
Disinfection of final effluent has been carried out with e.g.
CHLORINE or OZONE. In at least one plant in the USA, dewatered sludge (50% solids) has been disinfected with IONIZING
RADIATION (dose: 1 Mrad from a 137 caesium gamma source).
[Bacterial activities in sewage treatment plants: AvL (1984)
50 665682. Environmental health engineering in the tropics:
Book ref. 216. Low-cost sewerage for developing countries:
Book ref. 217.]
sewer gas See ANAEROBIC DIGESTION.
sewer swab Syn. MOORE SWAB.
sex factor (1) A general term for a CONJUGATIVE PLASMID (sense
1). (2) Collectively, those genes in a conjugative plasmid which
specify conjugation (see e.g. RTF). (3) Syn. F PLASMID.
sex pheromone See PHEROMONE.
sex pili See PILI.
sex-ratio organism See SRO.
sexduction The transfer, by CONJUGATION (sense 1b), of chromosomal genes from one bacterium to another. Sexduction may
involve an HFR DONOR or a donor strain carrying a PRIME PLASMID; if the chromosome of the Hfr donor is mobilized by the F
PLASMID, or if conjugal transfer is promoted by an F plasmid,
the process is called F-duction.
sexually transmitted disease (STD) Any disease which can
be transmitted by intimate contact with e.g. genitals, mouth
or rectum. In addition to the classical VENEREAL DISEASES,
STDs include e.g. AIDS, HEPATITIS B, HERPES SIMPLEX, MOLLUSCUM
CONTAGIOSUM, NON-GONOCOCCAL URETHRITIS, TRICHOMONIASIS,
and genital warts (see PAPILLOMA), as well as parasitic infestation
by lice (crab) or mites (scabies, the itch).
Sezary syndrome (SS) A cutaneous T-cell lymphoma which
resembles but is distinct from ADULT T-CELL LEUKAEMIA;
HTLV-I provirus has been detected only rarely in SS, and does
not appear to be a primary causal agent. The neoplastic T cells
in SS may resemble those of ATL, but the nucleus is more
commonly cerebriform than multilobed; ATL and SS cells are
antigenically distinct and are functionally distinct in vitro [Book
ref. 106, pp. 275284].
SFFV See FRIEND VIRUS and RAUSCHER VIRUS.
sfiA, sfiB genes See SOS SYSTEM.
SFV SEMLIKI FOREST VIRUS.
SG Gower coefficient. In the comparison of two strains by
NUMERICAL TAXONOMY: an expression of the degree of similarity
in which the comparison involves both simple, discontinuous
data (e.g. + and , or 0 and 1) and continuous (quantitative)
data. (cf. entry SSM .)
SH-activated cytolysins THIOL-ACTIVATED CYTOLYSINS.
SH antigen Syn. HBsAg: see HEPATITIS B VIRUS.
shaded matrix In NUMERICAL TAXONOMY: a graphic representation of the interrelationships between the OTUs in a given study.
It is a triangular tabulation, the ordinate and abscissa each consisting of a complete list of designations of the OTUs under
study; the degree of mutual similarity between the OTUs in any
given cluster is indicated by the intensity of shading: the highest
degree of similarity corresponds to the darkest shading.
flocs [see Microbiology (1998) 144 519528]. [Microbial communities in sewage treatment plants: FEMS Ecol. (1998) 25
205215.]
In this process, the sludge increases in mass due to microbial
growth; following sedimentation, most is removed for disposal,
some being retained for treating the next batch of sewage.
The biological aerated filter (BAF) is a more efficient
approach to aerobic secondary treatment. It consists of a
submerged bed of fine granular material coated with biofilm; the
sewage passes downwards through the bed while air is pumped
in at the base of the bed. Because the granules are small, the
system can function as a mechanical filter (for fine particulate
matter) as well as allowing mineralization of dissolved organic
matter. The biofilm in a BAF contains up to five times more
biomass than that in a trickle filter of equivalent size so that,
for a given treatment capacity, a BAF can be much smaller.
Appropriate flow conditions in the BAF allow adequate
aeration and the establishment of nitrifying bacteria in the
biofilm. The importance of this is that NITRIFICATION facilitates
the elimination of nitrogen from sewage; thus, if nitrification
can be achieved it can be followed by DENITRIFICATION. To
encourage denitrification the BAF can be operated anaerobically;
much of the nitrogen in sewage can therefore be eliminated
by operating aerobic and anaerobic BAF reactors in series.
[Combined nitrificationdenitrification: FEMS Reviews (1994)
15 109117.]
Anaerobic treatment is useful for sewage containing a high
proportion of solids (e.g. farm waste, sludge from the activated
sludge process). In this process (ANAEROBIC DIGESTION), the
stirred sludge is digested in a tank maintained at ca. 35 C. This
reduces the bulk of sludge, giving a less offensive material which
can be de-watered in sludge-drying beds; much of the carbon is
eliminated as methane (which can supply most or all of the
energy needs of the plant). (See also IMHOFF TANK.)
Anaerobic treatment can also be used e.g. for wastewater
containing terephthalic acid (1,4-benzenedicarboxylic acid) and
its isomers compounds used in the manufacture of polyester
products and plastic bottles; in one study, organisms associated
with the anaerobic granular sludge system included a high proportion of unidentified bacteria of the d-Proteobacteria and a
number of archaeans related to Methanosaeta and Methanospirillum [Microbiology (2001) 147 373382].
Tertiary treatment is sometimes used to reduce still further
the BOD of the effluent; this may be needed e.g. if discharge of
final effluent to a river is associated with a low dilution factor.
To reduce the amount of fine particulate matter, the effluent can
be passed through a microstrainer : a hollow cylinder of finemesh stainless steel fabric, closed at one end, which rotates on a
horizontal axis; effluent is pumped into the cylinder, and strained
effluent passes out through the mesh material retained on the
inner surface of the cylinder being constantly removed by jets
of water.
The Immedium filter is a sand filter in which the grain
size increases progressively from top to bottom; effluent flows
upwards through the filter. Other forms of filter, and grassland
irrigation, are also used for tertiary treatment.
The main purpose of tertiary treatment is often regarded as
the reduction of BOD by elimination of carbon from the effluent. However, removal of nitrogen (present mainly as ammonia
and nitrate) and phosphorus is also desirable in order to discourage the development of algal BLOOMS in the receiving waters.
(See also EUTROPHICATION.) The elimination of nitrogen was
considered earlier (see BAF). Phosphorus has been removed
701
shadow-casting
is centrifuged onto a culture of fibroblasts and the preparation subsequently stained with fluorescent monoclonal antibodies
specific for the 72 kDa phosphoprotein product (p72) of an
immediate-early gene.
shellfish diseases See e.g. CRUSTACEAN DISEASES and OYSTER
DISEASES.
shellfish poisoning A form of FOOD POISONING which results from
the consumption of shellfish (molluscs, crustacea) contaminated
with toxins or pathogens. Aquatic bivalve molluscs (clams, cockles, mussels, oysters etc) obtain their food by filtering microscopic organisms from the ambient water. Any human pathogens
present in the water can thus be concentrated in the bodies of
the shellfish and can cause disease when these are eaten by
humans. Pathogens transmitted in this way include e.g. HEPATITIS
A virus, enteroviruses, parvovirus-like agents (see FOOD POISONING (i)), and salmonellae (including S. typhi ); such pathogens
typically derive from sewage, whereas Vibrio parahaemolyticus
(see FOOD POISONING (h)) is a natural inhabitant of brackish and
marine waters. Gastropod molluscs (e.g. whelks, winkles) and
crustacea (e.g. lobsters, prawns) are not filter-feeders but may
nevertheless become contaminated with pathogens which may
be derived from the natural habitat of the animal (as e.g. in the
case of V. parahaemolyticus) or may be introduced during the
handling and processing of the shellfish (as e.g. in the case of
staphylococci). (See also FISH SPOILAGE.)
Paralytic shellfish poisoning (PSP, mussel poisoning) is a
severe, often fatal condition resulting from the consumption of
shellfish (commonly mussels or clams) which have themselves
consumed neurotoxin-forming dinoflagellates (e.g. Gonyaulax
spp) and accumulated the toxin(s) e.g. SAXITOXIN in their
tissues. (See also RED TIDE.) Symptoms of PSP (caused by
saxitoxin) typically include diarrhoea, fatigue, and a tingling
sensation beginning around the face and spreading to the arms,
fingers, and toes; later, numbness may develop, followed by
weakness, paralysis, and death (usually within 12 hours) from
respiratory paralysis. (cf. CIGUATERA.)
sherry See WINE-MAKING.
ShET2 enterotoxin See EIEC.
Shewanella A genus of bacteria proposed to include Alteromonas
hanedai (S. hanedai), A. putrefaciens (S. putrefaciens), and
strains of barophilic bacteria (see BAROPHILE) isolated from deepsea waters (S. benthica) [SAAM (1985) 6 171182; name validation: IJSB (1986) 36 354356]. (cf. ALTEROMONAS.)
shield cell (algol.) See CHAROPHYTES.
shift up, shift down (Refers to) a change in (experimental)
conditions which causes the growth rate of a microorganism
to increase (shift up) or decrease (shift down).
ShigaKruse bacillus Shigella dysenteriae serotype 1.
shiga-like toxins See SHIGA TOXIN.
shiga toxin A protein toxin, produced by strains of Shigella
dysenteriae, which apparently causes at least some of the
symptoms of (bacillary) DYSENTERY; the toxin is cytotoxic in
vivo, and is also toxic for some types of cultured cells (e.g.
HeLa).
The shiga holotoxin consists of an A subunit associated with
a pentameric ring of B subunits. The holotoxin binds, via B
subunits, to glycolipid receptor sites on the target cell; these
receptors globotriosylceramide (Gb3 ) are found e.g. in the
membrane of endothelial cells (cells that line blood vessels).
Shiga toxin is reported to be active against e.g. endothelial cells,
colonic/ileal epithelial cells, and B lymphocytes expressing the
CD77 ANTIGEN.
On uptake of toxin by a cell, the A subunit undergoes
proteolytic cleavage, the (catalytic) part of the subunit remaining
sickener
siderophore itself (iucAiucD) and its (outer membrane) receptor
protein (iutA) are carried by many COLV PLASMIDS, although the
system may also be chromosomally encoded. [Plasmid-specified
aerobactin system: Book ref. 161, pp. 741757; characterization
of the iucA and iucC genes: JB (1986) 167 350355.] The products of the fhuB, fhuC and fhuD genes, located in the cytoplasmic
membrane and/or periplasm, may form a binding system for the
uptake of iron by aerobactin and other hydroxamate siderophores
[JGM (1992) 138 597603].
In Escherichia coli, the outer membrane receptor for aerobactin, the IutA protein, can also bind CLOACIN DF13. In E. coli,
the aerobactin and enterobactin systems can be induced independently [Inf. Immun. (1986) 51 942947]; both systems apparently require the TONB PROTEIN for transport into the periplasm
[JGM (1992) 138 597603].
Other hydroxamate siderophores include e.g. coprogen (produced by many fungi); ferrichrome (formed e.g. by species
of Aspergillus, Neurospora and Ustilago): a cyclic hexapeptide consisting of a glycine tripeptide and a tripeptide of d-N acetyl-L-d-N -hydroxyornithine; ferrioxamines and DESFERRIOXAMINE (formed e.g. by certain bacteria); NOCARDAMINE; and the
terregens factor (a growth requirement of e.g. Arthrobacter spp).
For extracellular growth, the pathogen Mycobacterium tuberculosis uses a peptide siderophore, EXOCHELIN, and a cell-wallassociated lipophilic compound: MYCOBACTIN; exochelin appears
to obtain iron from SIDEROPHILINS and to pass it to mycobactin
for internalization.
Certain siderophores, e.g. parabactin, have been found to be
active, in vitro, against a murine leukaemia cell line and against
herpes simplex type 1 virus [TIBS (1986) 11 133136].
(See also PYOVERDIN.)
SIDS SUDDEN INFANT DEATH SYNDROME.
sIg Any immunoglobulin at the surface of a B LYMPHOCYTE.
sIgA Secretory IgA (see entry IgA).
sigatoka disease Syn. BANANA LEAF SPOT.
sigF gene See SIGMA FACTOR.
sigla Plural of SIGLUM.
siglum A designation consisting of letters (particularly initial
letters) and/or other characters. Some sigla are acronyms.
s (superhelix density) See DNA.
s factor (sigma factor) A protein which can bind to a DNAdependent RNA POLYMERASE (RPase) core enzyme and confer on
it the ability to initiate TRANSCRIPTION from a particular type of
PROMOTER.
Cells typically or always encode more than one type of sigma
factor, and different types of sigma factor generally confer on
the RNA polymerase the ability to transcribe (in vivo) from
different promoters; by synthesizing particular type(s) of sigma
factor, at appropriate times, the cell can thus control expression
of particular gene(s).
In Escherichia coli the main sigma factor is s70 (MWt
70000) encoded by gene rpoD; an RPase holoenzyme containing s70 (Es70 ) can initiate transcription from most promoters in
the E. coli genome sometimes in association with positive regulatory factors (as e.g. in CATABOLITE REPRESSION). Other sigma
factors in E. coli include e.g. s32 (RpoH, formerly HtpR: see
HEAT-SHOCK PROTEINS) and s60 (the NtrA protein: see NTR GENES).
There are many examples of the way in which the timing of
gene expression is controlled by the activity of particular sigma
factor(s). In E. coli, assembly of the FLAGELLUM from a number
of different proteins is a highly organized process in which
components are added in strict sequence the corresponding
genes being expressed in a way that reflects this sequence.
signal hypothesis
Thus, class III genes are expressed only after genes of classes
I and II, and the expression of class III genes depends on
synthesis of a sigma factor encoded by the fliA gene; however,
even when FliA has been synthesized, this sigma factor is
temporarily inactivated by an anti -s factor (FlgM, product of
gene flgM ) until the basal body and hook of the flagellum have
been completed completion of the hook apparently acting as a
signal that allows release of FlgM and consequent transcription
of the class III genes. [Genetic control of flagellar assembly:
Cell (1995) 80 525527.]
The E. coli sigma factor ss (encoded by rpoS ) was once
associated solely with stationary-phase events but is now known
to be involved in the regulation of various responses to stress
under log-phase, as well as stationary-phase, conditions [Mol.
Microbiol. (1996) 21 887893]. Under in vitro conditions,
either Es70 or Ess can be used for transcription from some
promoters, but, in vivo, many promoters exhibit specificity
for one of the two holoenzymes Es70 or Ess ; studies on
sigma factor specificity in the osmY gene have indicated that
specificity for ss in this gene is influenced strongly (perhaps
even determined) by three global regulators the cAMPCRP
complex (see CATABOLITE REPRESSION), the integration host factor
(IHF) and the leucine-responsive regulator protein (Lrp) which
preferentially inhibit Es70 -dependent expression from the osmY
promoter [EMBO (2000) 19 30283037].
Expression of the rpoS gene is reported to be regulated by the
HU PROTEIN [Mol. Microbiol. (2001) 39 10691079] and also by
a small, novel RNA molecule which interacts with rpoS mRNA
and relieves the inhibitory activity of a stem- and-loop structure
[Mol. Microbiol. (2001) 39 13821394].
In vegetative cells of Bacillus subtilis the major sigma factor
is s43 (formerly called s55 ; encoded by gene rpoD); this sigma
factor shows some homology with the E. coli s70 and recognizes
the same class of promoters. There are also a number of minor
sigma factors. A sigma factor may be present at low levels during
normal growth but up-regulated under appropriate conditions.
For example, sH (encoded by gene spo0H ) is up-regulated
during the initiation of sporulation in Bacillus subtilis as a
consequence of repression of abrB by Spo0AP (see figure (a)
in ENDOSPORE). Later in the initiation process, the sporulationspecific sigma factors sE (formerly s29 ; encoded by spoIIG) and
sF are synthesized to promote the next stage of sporulation.
The Es28 of B. subtilis can initiate transcription at E. coli
heat-shock promoters.
In B. subtilis, many of the genes and operons so far investigated have two or more overlapping or adjacent promoters which
are usually specific for RPase holoenzymes containing different
sigma factors; this presumably allows control of gene expression under various conditions and/or during different stages of
development.
In Mycobacterium tuberculosis, the discovery of a gene (sigF )
[PNAS (1996) 93 27902794] encoding a protein homologous
to a sporulation-specific sigma factor in Streptomyces coelicolor
has provided some evidence in support of the hypothesis that
latency (persistence) in this pathogen is associated with the
presence of a spore-like state. [Mechanisms of latency in
M. tuberculosis: TIM (1998) 6 107112.]
Certain bacteriophages encode sigma factors that are necessary for the expression of some of their genes: see e.g. BACTERIOPHAGE SPO1 and BACTERIOPHAGE T4 (gp55).
In some cases, the expression of a sigma factor results from
up-regulated translation of its mRNA (rather than increased transcription of the gene). In E. coli, for example, the increase in
signal peptidase
reticulum (see SIGNAL HYPOTHESIS); an SRP contains six polypeptides together with a 7S RNA which is essential for function
[Nature (1982) 299 691698].
In prokaryotes: a particle involved in the translocation of
certain proteins across the cytoplasmic membrane (see type II
systems in PROTEIN SECRETION).
signal sequence See SIGNAL HYPOTHESIS.
signal transducers and activators of transcription (STATs) See
CYTOKINES.
signal transduction pathway See TWO-COMPONENT REGULATORY
SYSTEM.
signature-tagged mutagenesis A form of TRANSPOSON MUTAGENESIS which can be used to detect those genes, in a pathogen,
which are necessary for the pathogens growth within the host
organism. The principle of signature-tagged mutagenesis is outlined in the figure. (See also IVET.)
signet-ring stage (of Plasmodium) See PLASMODIUM.
significant bacteriuria BACTERIURIA in which a sample contains
potentially pathogenic bacteria in numbers high enough to
indicate a URINARY TRACT INFECTION; the numbers of such
bacteria must be significantly higher than those which might
be expected to occur from contamination of the sample.
In the absence of infection, an MSU (taken correctly) should
contain no more than 104 (commonly <103 ) contaminating
bacteria/ml, and these contaminants will typically consist of
several species giving rise to different types of colony on the
culture plate.
By contrast, counts greater than 105 /ml usually consisting
of one species (but sometimes two species) are likely to
indicate an infection of the urinary tract; note that counts at this
level may not be obtained after chemotherapy with an effective
agent. (Note also that an inappropriately high count may be
obtained if the specimen of urine has been stored, prior to
culture, under conditions which allow multiplication of bacteria;
ideally, the sample should be examined promptly.)
In some cases a significant bacteriuria can be demonstrated in
an asymptomatic patient prior to development of pyelonephritis.
Conversely, some samples from patients with a urinary tract
infection may give low-level counts. Thus, interpretation of
counts must reflect the overall clinical picture.
Some pathogens can persist intracellularly in the facet cells
of bladder epithelium (see UPEC), so that counts of bacteria in
urine samples may not necessarily reflect the level of pathogenic
organisms within the urinary tract.
[Automated detection of significant bacteriuria by flow cytometry: JCM (2000) 38 28702872.]
silage A feed for animals (particularly ruminants) which is made
by the anaerobic storage of large masses of finely chopped
grasses, legumes or other green crops. Bacteria mainly Lactobacillus spp which are present on the vegetation and/or in
the storage vessel (silo) metabolize the plant sugars (especially
glucose, fructose and sucrose) primarily by a LACTIC ACID FERMENTATION, thereby causing a rapid fall in pH; the low pH
(ca. 4.0) inhibits various putrefactive organisms (particularly
Clostridium spp), thus helping to preserve the nutrient value
of the crop, and inhibits the growth of Listeria monocytogenes
(see also LISTERIOSIS). (cf. AIV PROCESS.) Ensilage may take ca.
14 months.
The crop to be ensiled is harvested when its nutrient value
is high, and before ensilage it may or may not be wilted (i.e.,
allowed to lose water); wilting to a dry-matter level (DM level)
of ca. 300 g/kg is usually sufficient to inhibit the growth of
putrefactive clostridia which need a minimum WATER ACTIVITY
Infect test
animal
all transposons in
the pool; then use
Replica 1
(clones)
Replica 2
probing Replica 2
SIGNATURE-TAGGED MUTAGENESIS: a method for identifying virulence-associated genes in a pathogen (general principle).
A unique sequence (tag) of about 40 base-pairs in length is inserted into each of a population of transposons, i.e. the tag in each transposon
is different from that in all the other transposons. Each tag is flanked, on both sides, by a short primer-binding site these sites being the same
in all transposons. The transposons are used to mutagenize cells of the pathogen, and they insert, randomly, into different genes in different
cells.
The mutagenized cells are plated to form individual colonies; a given colony consists of a clone of mutant cells, each containing the same
uniquely tagged transposon in the same gene. A number of colonies are chosen, and an inoculum from each colony is arrayed, separately, in
a microtitre dish. (The dish shown in the diagram has 30 wells, but larger dishes are normally used.) Two replica blots of the array are made
on membranes (for subsequent DNA hybridization studies); in these blots the cells are lysed and their chromosomal DNA is exposed and fixed
to the membrane in single-stranded form.
Cells are taken from each of the wells and pooled. The pool is used in two ways. First, it provides an inoculum for infection of the test
animal. Second, cells from this (input) pool are lysed, and PCR is used with labelled primers to amplify the unique tags of all transposons
in the pool. The amplified, labelled tags are then used as probes on one of the replica blots; in this blot (Replica 1), each (unique) tag should
hybridize with the DNA from cells containing the corresponding transposon. This pre-screening process (on Replica 1) checks for efficient
amplification of each unique tag in the pool. (The need to pre-screen may be avoidable if a set of dedicated tags is used [TIM (1998) 6 51].)
The pathogen is recovered from the test animal by plating an appropriate specimen. The resulting colonies are pooled (forming the
recovered pool), and PCR is used (with labelled primers) to amplify the tag from each clone in this pool. The amplified, labelled tags are then
used to probe the second replica blot (Replica 2). (Continued on page 708.)
707
silent mutation
higher than that required by lactic acid bacteria. The vegetation
is chopped into pieces ca. 2.5 cm in length and may be
treated with additives such as (a) a bacterial culture (usually
certain Lactobacillus spp) to augment the natural microflora,
(b) a carbohydrate (e.g. molasses) to augment the plant sugars,
and/or (c) formic acid, which e.g. can quickly establish a low
pH suitable for the growth of lactic acid bacteria. (At ca.
pH 5, formic acid is much more inhibitory to clostridia and
enterobacteria than it is to lactic acid bacteria; it thus tends
to promote the correct, i.e., lactic acid, fermentation.) The
chopped/treated vegetation is packed into the silo. When the silo
is sealed, microbial metabolism quickly results in anaerobiosis.
Organisms dominant in fermenting silage include homoand heterofermentative species of LACTOBACILLUS, particularly
L. brevis, L. buchneri, L. curvatus and L. plantarum; other
organisms may include e.g. Enterococcus faecium, Lactococcus
lactis, and species of Pediococcus and Leuconostoc. (Enterobacteria and Bacillus spp can be dominant during the first day or
so in vegetation of relatively low DM and high pH.) The heterofermentative organism L. brevis ferments glucose or fructose
to lactic and acetic acids, but does not form ethanol since it
apparently lacks aldehyde dehydrogenase [see Appendix III(b)];
in this species the excess reducing power can be used to reduce
exogenous fructose to mannitol (cf. RESPIRATION). Interestingly,
the mannitol and acetic acid formed by L. brevis can be used
as substrate and electron acceptor, respectively, by the homofermentative species L. plantarum [Food Mic. (1986) 3 7381].
When the silage is eventually removed from the silo it
can undergo aerobic deterioration if left uneaten; particularly
prone to such deterioration is silage made from overwilted
vegetation or made in a non-airtight silo i.e., circumstances
which tend to increase the aerobic silage microflora. Organisms
particularly associated with aerobic deterioration include yeasts
(e.g. Hansenula, Pichia, Saccharomyces), other fungi (e.g.
Aspergillus, Byssochlamys, Fusarium, Geotrichum and Mucor ),
and Bacillus spp. The addition of certain compounds (e.g.
propionic acid) to the vegetation at the beginning of ensilage can
reduce subsequent aerobic deterioration in the finished silage.
Sorbic acid can have a similar effect.
Various additives are used e.g. to increase the efficiency of
the process and/or to enhance the performance of animals fed
on the silage. One common additive includes strains of lactic
acid bacteria that carry out a homolactic fermentation. Ideas
for improved additives include (i) strains of lactic acid bacteria
particularly suited to specific target crops; (ii) lactic acid bacteria
that carry out a heterolactic fermentation the volatile fatty
acids inhibiting growth of fungi when the silage is exposed to air
at feeding time; (iii) genetically engineered lactic acid bacteria
which can utilize polysaccharides in those silage crops with low
levels of soluble carbohydrates [new trends in silage additives:
FEMS Reviews (1996) 19 5368].
SIGNATURE-TAGGED MUTAGENESIS (continued) Considering the original, mutagenized cells in the input pool, the cells of interest are those
which, through a (transposon-mediated) mutation, are unable to grow within the test animal, i.e. cells whose virulence has been lowered; such
cells will be absent, or few in number, in the recovered pool (compared with those cells which were able to grow normally in the test animal).
Hence, the signature tags of these virulence-attenuated cells will be present in the input pool but absent (or rare) in the recovered pool;
consequently, such cells can be identified by hybridization on Replica 1 but an absence of (or weak) hybridization on Replica 2 (see figure). (If
dedicated tags had been used, virulence-attenuated cells would be identified by the absence of hybridization on a single blot.)
In a given virulence-attenuated clone, the relevant gene (identifiable from the inserted transposon) can be isolated, cloned and sequenced
for further study.
Reproduced from Bacteria, 5th edition, Figure 8.22, pages 218219, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN
0471-98880-4) with permission from the publisher.
708
simian virus 40
for exogenous retroviruses which infect the T cells of monkeys
and other subhuman primates. STLV-I (formerly STLV) is
closely related to HTLV-I (see HTLV); it infects Old World
monkeys and apes, and can cause lymphomas in e.g. macaques.
STLV-III has been isolated from rhesus monkeys (Macaca
mulatta) and African green monkeys (Cercopithecus aethiops)
and appears to be closely related to the human AIDS virus; a
virus similar to STLV-III can apparently infect humans, and it
has been suggested that the AIDS virus and STLV-III may have
had a common origin [Science (1986) 232 238243]. (cf. SIMIAN
AIDS.)
simian virus 40 (SV40; vacuolating agent) A virus of the genus
POLYOMAVIRUS. SV40 was originally isolated from kidney cells of
the rhesus monkey (Macaca mulatta) and is common (in latent
form) in such cells; early polio and adenovirus vaccines prepared
in rhesus monkey kidney cells were frequently contaminated
with SV40. (See also MASTADENOVIRUS.) In kidney cells from the
African green monkey (Cercopithecus aethiops) SV40 causes
CPE, including characteristic vacuolation of the cytoplasm.
SV40 is usually non-pathogenic in its natural host, but can
induce fibrosarcomas and gliomas in newborn rodents (though
not in immunocompetent adult animals): see POLYOMAVIRUS for
details.
similarity matrix See S MATRIX.
Simkania negevensis See SPLIT GENE (bacterial).
Simmons citrate agar KOSERS CITRATE MEDIUM incorporating
BROMTHYMOL BLUE (0.008%) and agar (1.52.0%).
Simonsiella A genus of GLIDING BACTERIA (see CYTOPHAGALES)
which occur in the oral cavity in man and other vertebrates.
The organisms are flat filaments (ca. 24 m in length), each
composed of elongated cells arranged side-by-side; the outer
face of each terminal cell is rounded. Gliding occurs in a
direction parallel to the long axis of the filament. Metabolism:
chemoorganotrophic.
Simonsiellaceae See CYTOPHAGALES.
simple matching coefficient See entry SSM .
Simplexvirus See ALPHAHERPESVIRINAE.
Sin Nombre virus See HANTAVIRUS.
SIN virus SINDBIS VIRUS.
Sindbis virus (SIN virus) An ALPHAVIRUS which occurs in
Africa, Asia, Australia and Europe; it is apparently maintained
primarily in birds and is transmitted by mosquitoes which feed
on birds (e.g. Culex univattatus in Africa). Other vertebrates
can be infected, and the virus is occasionally associated with
human illness characterized by arthralgia and a maculopapular rash (Sindbis fever); human diseases caused by Sindbis or
related viruses are known as Karelian fever in the former USSR,
Ockelbo disease in Sweden, and Pogosta disease in Finland. (See
TOGAVIRIDAE for replication cycle etc.)
sinefungin An ANTIBIOTIC (obtained from Streptomyces griseolus) which has antifungal, antiprotozoal and antiviral activity; it
acts as an analogue of ornithine, inhibiting ornithine decarboxylase and hence putrescine formation.
single burst experiment A procedure for studying the lysis of
a single cell by a virus (e.g. to determine the BURST SIZE).
Essentially, a suspension of cells is infected with viruses and
then diluted such that each of a large number of aliquots has a
low probability of containing more than one virus-infected cell.
Following incubation and lysis, the pfu counts in the aliquots
can be statistically analysed e.g. to assess individual burst sizes.
The single burst experiment can also be used e.g. to investigate
recombination in bacteriophages, genetic analysis being made of
the phage progeny from a single bacterial cell coinfected with
two genetically distinct phages.
single diffusion
relatively low growth rates and protein content. Protein from
microalgae is inferior, nutritionally, to that of most other
microbial sources, and algal SCP has poor acceptability in taste,
colour, odour etc. The problem of indigestible algal cell walls
may be overcome by cultivating protoplasts or wall-less algae
(e.g. Dunaliella [AEM (1976) 31 602604] and Cosmarium
[AEM (1976) 32 436437]).
Production of SCP. Bacteria, yeasts and moulds are generally
cultured in well-aerated liquid media in a FERMENTER; typically,
the process is continuous (see CONTINUOUS CULTURE) with limiting carbon (C:N less than ca. 10:1) to minimize production of
storage compounds such as poly-b-hydroxybutyrate. Algae are
grown in batch or semi-continuous culture in ponds with large
surface areas. Yeasts and bacteria are harvested by centrifugation; in one process (Pruteen, see later) the bacteria are initially
agglutinated so that a more concentrated slurry can be fed to
the centrifuge thus increasing the efficiency of centrifugation.
Algae and moulds are harvested by filtration. The concentrated
biomass is washed, dried, and used either directly (e.g. in animal
feeds) or (for human consumption) its protein content may be
extracted and used as a nutrient supplement or as a functional
ingredient (e.g. to alter the texture of traditional foods).
Substrates. The choice of substrate involves considerations
such as cost, efficiency of utilization, continuity of supply, and
risk of toxic residues. There is, with some exceptions, a good
correlation between cell yield and substrate energy content for
substrates with heats of combustion up to ca. 11 kcal/g of
substrate carbon (approximately that of glycerol); above this
value cell yields do not increase [Book ref. 11, pp. 3334].
(a) High-energy substrates. Hydrocarbons, e.g. natural gas
(8095% methane) and n-alkanes (particularly C10 C23 ), can
be utilized very efficiently by certain bacteria and yeasts, and
the risk of microbial contamination is low owing to the inability of most potential contaminants to grow on these substrates.
However, hydrocarbons are poorly soluble in (aqueous) growth
media, and they may contaminate the final product although
methane, being gaseous, is easily eliminated; the n-alkanes can
be used in low concentrations in media containing ammonium
salts, phosphate, etc. A further (operational) problem is that
hydrocarbon substrates require high rates of oxygenation and
heat removal. Organisms which have been grown on hydrocarbons on an industrial scale include yeasts e.g. Yarrowia lipolytica (= Saccharomycopsis (Candida) lipolytica) and bacteria
(e.g. Pseudomonas spp which utilize waxy residues of crude
petroleum); they have been used as animal feeds. (See also
HYDROCARBONS and METHANOTROPHY.) [Hydrocarbons as substrates in industrial fermentations: Book ref. 155, pp. 643683.]
Methanol and ethanol are more soluble than hydrocarbons,
are readily available in pure form, and are easily removed from
the SCP but they are more expensive. Of organisms grown
on methanol, higher yields are given by those which use the
RMP PATHWAY rather than the SERINE PATHWAY. One commercial
product manufactured in the 1980s, was prepared by growing the obligate methylotroph Methylophilus methylotrophus on
methanol in an AIRLIFT FERMENTER. The product (Pruteen)
(Imperial Chemical Industries, UK) was marketed (ca. 70000
metric tons annually) as an animal feed, with purified carbon
dioxide as a by-product; the process was subsequently discontinued owing to a fall in the price of protein.
Owing to the high cost of ethanol, ethanol-derived SCP is
likely to be prepared only for human consumption; it includes
TORULA YEAST which has been produced at the rate of over
7000 tons annually by one American company.
single dimension
sinusitis Inflammation of one or more of the paranasal sinuses
often a complication of e.g. a COMMON COLD or a tooth infection. Symptoms include pain at the affected site, purulent
nasal discharge, and fever. Common causes of acute sinusitis are Haemophilus influenzae or Streptococcus pneumoniae
(or both); less commonly, S. pyogenes, Staphylococcus aureus,
Branhamella catarrhalis, or anaerobes (e.g. Bacteroides spp)
may be involved.
siomycin See THIOSTREPTON.
siphonaceous (siphonous) Refers to a tubular or vesicular,
coenocytic, basically aseptate algal thallus in which the cytoplasm (containing the chloroplasts, nuclei etc) forms a peripheral
layer around a large central vacuole. (Septa may separate reproductive structures from the rest of the thallus, and may be formed
in response to wounding.) According to species, a siphonaceous
thallus may be a simple or branched tube or vesicle (see e.g.
BOTRYDIUM and VAUCHERIA); in some algae (e.g. CODIUM) the
thallus is made up of a complex combination of such tubes and/or
vesicles. (cf. SIPHONOCLADOUS.)
siphonein See CAROTENOIDS.
siphonocladous Refers to a filamentous algal thallus which
is composed of multinucleate cells (as in e.g. CHAETOMORPHA, CLADOPHORA, RHIZOCLONIUM, SIPHONOCLADUS, VALONIA).
(cf. SIPHONACEOUS.)
Siphonocladus
A genus of marine, mainly tropical, siphonocladous green algae (division CHLOROPHYTA) in which the mature
thallus is erect with lateral branches.
siphonous Syn. SIPHONACEOUS.
siphonoxanthin See CAROTENOIDS.
sirenin See PHEROMONE.
siRNA See RNA INTERFERENCE.
sirodesmins See EPIPOLYTHIAPIPERAZINEDIONES.
sirohaem A HAEM (sense 1) which is the prosthetic group in
e.g. DESULFOVIRIDIN, in the sulphite and nitrite reductases of e.g.
Escherichia coli, and in certain IRONSULPHUR PROTEINS in green
plants.
Sirolpidium See LAGENIDIALES.
SIRS Systemic inflammatory response syndrome: specific symptoms (e.g. temperature >38 C or <36 C; white blood cell count
>12000/mm3 , <4000/mm3 or >10% immature forms) used to
define SEPSIS (sense 2) precisely. [Sepsis/SIRS: JAC (1998) 41
(suppl A) 1112.]
SIRS virus See BLUE-EARED PIG DISEASE.
sis An ONCOGENE originally identified as the transforming determinant of SIMIAN SARCOMA VIRUS; the v-sis product has an amino
acid sequence almost identical to that of human platelet-derived
growth factor (PDGF), and may cause transformation by mimicking PDGF [EMBO (1986) 5 15351541].
sisomycin 4 ,5 -DehydroGENTAMICIN C1a .
sister chromatid See CHROMATID.
site-directed mutagenesis Syn. SITE-SPECIFIC MUTAGENESIS.
site-specific mutagenesis The (in vitro) induction of MUTAGENESIS at a specific site in a given (target) DNA molecule.
In one method (D-loop mutagenesis), small fragments of
ssDNA, each corresponding to the site to be mutated, are
mixed (in vitro) with the full-sized supercoiled dsDNA target
molecules in the presence of RecA protein (q.v.) and ATP; under
these conditions the fragment invades the dsDNA, generating
a single-stranded D-loop which is susceptible to the ssDNAspecific mutagen BISULPHITE. The bisulphite-treated DNA is then
introduced into ung cells (see URACIL-DNA GLYCOSYLASE) by
TRANSFORMATION; during a subsequent round of DNA synthesis,
the uracil residues (generated from cytosine by the bisulphite)
pair with adenine, leading to GC AT transitions.
skin microflora
same or different molecules, with no synthesis or degradation of
DNA and without hydrolysis of phosphodiester bonds (i.e. the
reaction is independent of ATP and other energy sources). The
initial juxtaposition (synapse) of the sequences involves DNAbinding proteins; the two sequences are often identical, but in
some cases (e.g. the attB and attP sites in phage l integration)
they are dissimilar. Cuts are made at staggered sites in the two
strands of a given duplex, either concurrently or sequentially, and
similar cuts are made in the juxtaposed duplex; strand exchange,
between the duplexes, is followed by ligation.
Each particular type of SSR system involves a protein (a
recombinase) which recognizes specific sequences and appears
to mediate cutting, strand exchange and ligation; as well as a
recombinase, accessory proteins (e.g. the HU PROTEIN) may be
needed.
Recombinases are of two main types. One type is exemplified
by Tn3 resolvase (see TN3), the other by phage l integrase [TIG
(1992) 8 432439, and erratum in TIG (1993) 9 45].
A resolvase-type recombinase (encoded e.g. by Tn3, Tn21
and Tn552 ) forms an intermediate in which all four strands
are cut concurrently, with 5 phosphate bound to recombinase.
(Phosphateprotein binding conserves energy for subsequent
ligation.) The integrase-type recombinase (e.g. l Int, and the
lox /Cre system of BACTERIOPHAGE P1) cuts/joins strands pairwise;
this enzyme forms an intermediate equivalent to a Holliday
junction (see RECOMBINATION) in which only one pair of strands
has been exchanged.
Examples of SSR include: integration/excision of BACTERIOPHAGE l (q.v.); RECOMBINATIONAL REGULATION systems of
Salmonella and phage Mu; lox /Cre in BACTERIOPHAGE P1; the
resolvase of Tn3 (q.v.) and other transposable elements; gene
splicing; monomerization of plasmid dimers; some cases of plasmidchromosome interaction [JB (1992) 174 74957499]; and
insertion of the gene cassette into an integron [JAC (1999) 43
14].
Some authors regard transposition as a form of (nonconservative) site-specific recombination.
sitophilous Living or growing on food (especially cooked or
prepared food).
Sivatoshella See EIMERIORINA.
sixth disease Syn. EXANTHEM SUBITUM.
SJ Jaccard coefficient (sometimes spelt Jacquard coefficient). In
NUMERICAL TAXONOMY: a coefficient which is similar to SSM
(q.v.) but which is calculated on the basis of matching positive
characteristics; if a given characteristic is negative in both OTUs
it is discounted.
skeletal hyphae See HYPHA.
Skeletonema See DIATOMS.
skiaphilic (skiaphilous) Shade-loving.
skin microflora Human skin is a relatively hostile environment
for most microorganisms due e.g. to its low aw and the presence
of antimicrobial fatty acids released from sebum by the resident
flora. Resident bacteria normally include staphylococci (e.g.
S. epidermidis) and Propionibacterium acnes; these organisms
generally occur in scattered colonies on the skin and in the
pilosebaceous follicles [JGM (1984) 130 797801; 803807].
(See also ACNE.) Other organisms commonly present on skin
include yeasts (e.g. Malassezia spp), aerobic coryneforms, and
micrococci. Transient organisms depend e.g. on standards of
personal hygiene, and may include coliforms, streptococci,
pseudomonads etc.
A reduction in the numbers of microorganisms on the skin
may be desirable for various reasons (e.g. to prevent wound
G
T
M13
G
T
A
T
G
C
skin substantivity
Eflornithine (DL-a-difluoromethylornithine; DFMO) is used
against Trypanosoma (T.) brucei gambiense but is not effective
against T. (T.) brucei rhodesiense; this agent inhibits the enzyme
ornithine decarboxylase (ODC), thus inhibiting the synthesis
of trypanothione (see ARSENIC). The ability of eflornithine
to act therapeutically may depend on a slow turnover of
trypanosomal ODC (relative to that of mammalian ODC); this
appears to be the case with a cattle-infecting trypanosome [JBC
(1990) 265 1182311826]. Eflornithine is useful in late-stage
trypanosomiasis as it readily enters the CSF.
sleepy foal disease (shigellosis) An acute, usually fatal, septicaemic disease of newborn foals, caused by Actinobacillus
equuli. Infection may occur in utero or postnatally.
slide (microscope slide) A piece of flat, transparent, colourless
glass, about 75 25 1 mm, on which a specimen is placed
(or a SMEAR made) for microscopical examination; the specimen
may be overlaid with a COVER-GLASS. (The slide plus its specimen
is also referred to as a slide.) A suitably prepared specimen
(e.g. a fixed, dehydrated, cleared section of tissue) may be
made permanent by mounting it (e.g. in CANADA BALSAM) and
overlaying it with a cover-glass; when dry, the balsam cements
cover-glass to slide. (cf. CAVITY SLIDE, RING SLIDE.)
slide agglutination test Any agglutination test in which antigen
and antibody preparations are mixed and allowed to interact on
the surface of a slide; one or more dilutions of the antigen and/or
antibody preparations may be used in the test a given dilution
reacting with a standard amount of the other reactant. Such tests
are generally used only when detectable agglutination occurs
within minutes. (Agglutination may be detected e.g. by lowpower microscopical examination.)
slim disease In Africa: the name for a condition characterized by
a profound loss of weight and constant diarrhoea; the condition
is commonly (or always) AIDS.
slime bacteria Bacteria of the MYXOBACTERALES.
slime layer See CAPSULE.
slime moulds A category of eukaryotic organisms which typically have some fungus-like attributes (e.g., the production of
spores in or on fruiting bodies) and some animal-like attributes
(e.g., a phagocytic, amoeboid vegetative phase); as commonly
used, the term slime moulds refers specifically to the socalled true or acellular slime moulds (see MYXOMYCETES) and
the CELLULAR SLIME MOULDS. Taxonomically, these organisms
are variously classified together with certain other groups
of organisms as fungi (division MYXOMYCOTA), as protozoa
(mostly in classes of the RHIZOPODA the labyrinthulas and
thraustochytrids being placed in a separate phylum, Labyrinthomorpha), or as a distinct phylum (GYMNOMYXA) of the kingdom
PROTISTA (sense 2).
slimicide An antimicrobial agent used to inhibit slime-forming
organisms.
slipper animalcule The ciliate Paramecium.
slit sampler Any instrument, used for sampling the airborne
microflora, in which AIR is drawn in through a narrow slit onto
an adhesive collecting surface see e.g. HIRST SPORE TRAP.
slobber syndrome (vet.) See SLAFRAMINE.
slope (slant) (1) A solid medium which has been allowed to set
(in the case of e.g. agar or gelatin media) or which has been
inspissated (in the case of e.g. DORSETS EGG) in a diagonally
oriented test-tube or bottle. (See also BUTT and POTATO SLOPE.)
(2) A CULTURE prepared by the inoculation and incubation of
a slope (sense 1).
sloppy agar (semi-solid agar) See AGAR and MEDIUM.
slow-cycling rhodopsin (SCR) A RETINAL-containing protein,
small amounts of which have been detected in some of the strains
smoking
from caliciviruses. Sequencing data also show that SRSVs are
genetically diverse. Phylogenetic analysis indicates at least two
genogroups, each consisting of a number of genotypes; for
example, Norwalk virus, Southampton virus and Desert Shield
virus comprise genogroup 1, while three clusters (one consisting
of Hawii virus and Melksham virus) form genogroup 2.
[SRSVs (review): RMM (1997) 8 149155.]
small T antigen See POLYOMAVIRUS.
smallpox (variola major) An acute infectious human disease
caused by the variola major virus (see VARIOLA VIRUS). Infection
occurs by droplet inhalation and by direct contact with infected
persons or fomites. (Contaminated clothing, scabs etc can remain
infective for years.) Incubation period: 717 days. Typically,
symptoms begin abruptly, with fever, headache, nausea, and
muscle and joint pains; 24 days later the characteristic skin
lesions appear. The lesions are most numerous on exposed
parts of the body (face, hands etc); they begin as macules,
becoming vesicular, then pustular, finally drying to form thick
crusts which eventually drop off, leaving scars (pockmarks).
The disease may be fatal; recovery is followed by long-term
immunity. Other forms of the disease occur. Haemorrhagic
smallpox is the most severe, with generalized haemorrhages
and mortality rates of ca. 100%. Variola sine eruptione is
a mild, feverish illness (without skin lesions) resembling the
prodromal stage of classical smallpox; it occurs mainly in
vaccinated individuals. Alastrim (variola minor, Kaffir pox,
amaas) is a mild form resembling classical smallpox; it is caused
by the variola minor virus. Complications of smallpox include
e.g. secondary bacterial infection of skin lesions followed by
septicaemia; lesions in the eyes may lead to blindness. Lab.
diagnosis: identification and/or culture of the virus from vesicle
fluid, smears from skin lesions etc (see also GUARNIERI BODIES);
serological tests (e.g. precipitin test, CFT). Vaccines against
smallpox contain live VACCINIA VIRUS which is injected into
the skin to establish a localized viral infection in which a
smallpox-like lesion forms at the vaccination site. Complications
of vaccination include e.g. eczema vaccinatum (see ECZEMA),
post-vaccinal ENCEPHALITIS, and generalized vaccinia. Immunity
induced by vaccination wanes after several years, although an
allergic sensitivity to viral proteins may persist.
In the past, smallpox occurred in epidemics and pandemics
throughout the world, with enormous suffering and loss of life.
A world-wide eradication programme (based on vaccination,
isolation of cases etc), launched by the WHO in 1967, has
led to the complete extinction of the disease in nature the
first disease to have been conquered on a global scale. The
last recorded naturally acquired cases occurred in October 1975
(variola major) and October 1977 (variola minor). Eradication
was possible since there is no asymptomatic human carrier state
and apparently no animal reservoir (cf. MONKEYPOX).
Smc protein See CELL CYCLE (b).
smear (film) Any material (e.g. bacterial culture, wound exudate)
prepared for microscopical examination as a thin film on a SLIDE;
a smear is often dried, fixed (see e.g. FLAMING), and stained prior
to microscopical examination.
SMEDI viruses See ENTEROVIRUS.
smf SODIUM MOTIVE FORCE.
smoking (of meats, fish) A method of FOOD PRESERVATION in
which the foodstuff is exposed to smoke for hours or days;
smoking has a drying effect, lowering the WATER ACTIVITY and
raising the salt concentration of the food. Wood smoke contains
various phenolic, cresylic and aldehyde components which have
antibacterial and antifungal properties.
soft rot
snRNAs function in the nucleus in the form of small nuclear
ribonucleoprotein particles (snRNPs or snurps). Some proteins
are common to several snurps, and some snurps contain more
than one snRNA (e.g. U4 and U6 both occur apparently basepaired together in the same snurp). Snurps are believed to play
important roles in mediating and regulating post-transcriptional
RNA processing events: e.g. the splicing of introns from nuclear
pre-mRNA (see SPLIT GENE (a)). [Nature (1985) 316 105106;
functions for snRNAs in yeast: TIBS (1986) 11 430434;
conservation of U-snRNPs in fungi, plants and vertebrates:
EMBO (1987) 6 469476.] (cf. SCRNA.)
snRNP See SNRNA.
snurp See SNRNA.
SnyderTheilen feline sarcoma virus See FES.
soaps (as antimicrobial agents) In general, soaps (sodium or
potassium salts of long-chain fatty acids) have little or no intrinsic antimicrobial activity, but their surfactant properties can help
to reduce the number of microorganisms on the skin. Some
soaps are given positive antimicrobial properties by the incorporation of certain antiseptics (see e.g. BISPHENOLS); carbolic soap
contains phenol, and some antiseptic soaps contain TCC (see
CARBANILIDES). Critical concentrations of soap are needed for the
activity of some disinfectants (e.g. Lysol see PHENOLS). Some
antimicrobial agents (e.g. QUATERNARY AMMONIUM COMPOUNDS)
may be inactivated by soaps.
SOB system See SOS SYSTEM.
sobemoviruses (southern bean mosaic virus group) A group of
ssRNA-containing PLANT VIRUSES, each of which has a relatively
narrow host range; transmission occurs via beetles, via seeds
(in some hosts), and mechanically. Type member: southern
bean mosaic virus (SBMV); other member: turnip rosette
virus. Possible members include e.g. blueberry shoestring virus,
cocksfoot mottle virus, and rice yellow mottle virus.
Virion: icosahedral (ca. 30 nm diam.) stabilized by divalent cations. The structure of SBMV is similar to that of
TOMBUSVIRUSES, but the coat protein (MWt ca. 30000) lacks a P
domain. Genome: one molecule of linear positive-sense ssRNA
(MWt ca. 1.4 106 ); the 3 end is neither polyadenylated nor
tRNA-like, and the 5 end is associated (in SBMV and TRV)
with a small protein which is necessary for infectivity. Virions occur in both nucleus and cytoplasm in infected plant cells,
sometimes forming crystalline arrays in the cytoplasm.
SOD SUPEROXIDE DISMUTASE.
Sodalis A genus of Gram-negative bacteria of the family Enterobacteriaceae which occur as intra- and intercellular symbionts in
various tissues of the tsetse fly (GLOSSINA) (but which can also
be grown in vitro). Studies on the genome of S. glossinidius
have indicated that, compared with the genome of Escherichia
coli, many of the genes concerned with energy metabolism
and with the assimilation of carbon compounds appear to be
missing; it was suggested that this may indicate an adaptatin to
the use of those energy sources which are available in blood
[genome size and coding capacity of S. glossinidius: JB (2001)
183 45174525].
(See also WIGGLESWORTHIA and WOLBACHIA.)
sodium azide See AZIDE.
sodium dodecyl sulphate See SDS-PAGE.
sodium motive force (smf) The energy associated with a transmembrane electrochemical gradient of sodium ions; smf is analogous to proton motive force (pmf) (see CHEMIOSMOSIS).
In some organisms smf is generated by Na+ /H+ antiport
and is used as a driving force for certain TRANSPORT SYSTEMS;
for example, the Na+ / melibiose symport system is used by
soft swell
field; the resonating metal is mechanically linked to a metal
probe (a cylindrical metal rod) which dips into the liquid and
acts as the transmitter of sound energy. The sound waves used
are often between 10 kHz and 25 kHz with amplitudes of ca.
1050 m. (1 kHz = 1 kc/s = 1000 cycles/second.)
sonifier Syn. SONICATOR.
sooty bark A disease of Acer spp (maple, sycamore) caused by
Cryptostroma corticale; the bark of standing trees peels away
to reveal dark-brown masses of conidia. (See also MAPLE BARK
STRIPPERS DISEASE.)
sooty moulds Fungi of the family Capnodiaceae and of certain
other families of the order DOTHIDEALES. The organisms grow
epiphytically, utilizing HONEYDEW, and form dark, spongy,
hyphal mats on the surfaces of certain plants. Genera: e.g.
Capnodium, Scorias. (cf. BLACK MILDEWS.)
sop locus See PARTITION.
SopA protein See PROTEIN SECRETION (type IV systems).
SopB See FOOD POISONING (Salmonella).
sophorolipids Extracellular glycolipid BIOSURFACTANTS produced
by Torulopsis sp during growth on hydrocarbons; they consist
of sophorose covalently linked to the hydroxy group of a
hydroxy fatty acid.
sophorose b-D-Glucopyranosyl-(1 2)-D-glucopyranose an
effective inducer or certain CELLULASES. It occurs e.g. in certain
plant glycosides and as an impurity in commercial glucose.
soralium (lichenol.) A delimited mass of soredia (see SOREDIUM)
present on the thallus in certain lichens. Soralia may occur in
positions and forms which are characteristic for a given lichen
species: they may be e.g. marginal (at the edges of the thallus),
capitate (at the tips of lobes or branches), laminal (on the upper
or lower surface of the thallus), etc.
Sorangium See MYXOBACTERALES.
sorbates See SORBIC ACID.
sorbic acid (CH3 (CH=CH)2 COOH) An antibacterial and antifungal ORGANIC ACID used (as the free acid or e.g. as the potassium salt) as a PRESERVATIVE (e.g., in soft drinks, wines, pickles,
cheese, pharmaceuticals). It has been reported that both dissociated and undissociated forms of sorbic acid have antimicrobial
activity, but that organisms differ greatly in their susceptibilities [JAB (1983) 54 383389]. Potassium sorbate (12% w/v)
has been shown to reduce the germination rate of Clostridium
botulinum type E endospores under acidic conditions [AEM
(1982) 44 12121221].
sorbitol (glucitol) The POLYOL corresponding to glucose; Dsorbitol may be obtained e.g. by reduction of D-glucose, Dfructose or L-sorbose (see also ASCORBIC ACID). Sorbitol occurs
naturally e.g. in certain plants, including a few unicellular green
algae and a single red alga (Bostrychia scorpioides) [Book
ref. 37, pp. 165167]. D-Sorbitol is used e.g. as a food sweetener
for diabetics, and as a substrate in biochemical characterization
tests for bacteria (it is attacked by many species).
sorbitolMacConkey agar See EHEC.
sorbose fermentation A commercial FERMENTATION (sense 2)
in which D-sorbitol (see SORBITOL) is oxidized to the 2ketohexose L-sorbose by Acetobacter or Gluconobacter spp,
especially G. oxydans (Acetobacter suboxydans ). L-Sorbose is
used mainly as an intermediate in the manufacture of ASCORBIC
ACID.
Sordaria A genus of fungi (order SORDARIALES) which occur e.g.
on dung and soil; the organisms form brown or black ascospores
in persistent asci within dark perithecia see ASCOSPORE for
mode of spore discharge. Many species apparently do not form
conidia. S. fimicola is homothallic.
(2) (of fruit and vegetables) A type of rot, caused by pectinolytic organisms, in which fruit or vegetables degenerate into a
wet slimy mass. In acidic fruits (e.g. tomatoes, apples) soft rot is
commonly caused by pectinolytic fungi (e.g. species of Botrytis,
Penicillium, Rhizopus), while in non-acid fruits and vegetables
(e.g. potatoes, carrots) it is more commonly caused by bacteria
(e.g. species of Clostridium, Erwinia, Pseudomonas). (See also
BROWN ROT (sense 2) and PECTIC ENZYMES; cf. DRY ROT (2).)
soft swell See SWELL.
sog gene See CONJUGATION (1b) (i).
soil-borne wheat mosaic virus (SBWMV) A rod-shaped ssRNAcontaining virus which causes mosaic, stunting and yield
reduction in winter wheat in parts of Europe, Japan and the USA.
It is transmitted by the fungus Polymyxa graminis. Isolates of
SBWMV consist of at least two components, virion I (281300
nm long) and virion II (138160 or 92110 nm long) both of
which are necessary for infectivity. SBWMV has been classified
with the TOBAMOVIRUSES, but in view of its bipartite nature
and mode of transmission it has been proposed as the type
member of the furoviruses (fungus-borne rod-shaped viruses);
other members of the group may include e.g. BEET NECROTIC
YELLOW VEIN VIRUS, potato mop top virus, and peanut clump
virus [JGV (1984) 65 119127].
Solanum nodiflorum mottle virus (SNMV) See VELVET TOBACCO
MOTTLE VIRUS and VIRUSOID.
solfatara A dormant or decadent volcanic vent which (gently)
emits sulphurous gases.
solid-phase immunoelectron microscopy See SMALL ROUND
STRUCTURED VIRUSES.
Solorina
A genus of foliose LICHENS (order PELTIGERALES).
Photobiont: Coccomyxa, usually also with Nostoc. In e.g.
S. spongiosa the thallus consists of two distinct parts: rounded,
bright-green, Coccomyxa-containing lobes, each with a large,
central, pitcher-shaped apopthecium, and blue-black, Nostoccontaining squamules. In S. crocea, Nostoc occurs within the
thallus in a layer below the green algal layer. In S. saccata,
Nostoc occurs in discrete internal cephalodia. Solorina spp occur
mainly on calcareous soils, particularly at high altitudes.
solvent fermentation Syn. ACETONEBUTANOL FERMENTATION.
somatic (1) Refers to an assimilatory, vegetative (i.e., nonreproductive) structure or function.
(2) Refers to the body or main part of a cell. Thus, e.g. a
somatic antigen is a molecule which forms part of the body of
a cell, usually at the cell surface, rather than one which occurs
e.g. in a capsule or flagellum. (See e.g. O ANTIGENS.)
(3) Refers to common pili, i.e., FIMBRIAE, as opposed to PILI.
somatic cell hybridization See HYBRIDOMA.
somatic hypermutation See ANTIBODY FORMATION.
somatogamy The fusion of somatic (vegetative) cells or hyphae
involving PLASMOGAMY but not KARYOGAMY.
Sonacide An acidic GLUTARALDEHYDE solution.
Sonderia See TRICHOSTOMATIDA.
sonicate (1) (verb) To carry out SONICATION. (2) (noun) The
product of sonication.
sonication The use of audible sound waves, produced by a
SONICATOR, e.g. for the disintegration of cells in a liquid medium
(cf. ULTRASONICATION).
sonicator (sonifier) An instrument which provides sound energy
for SONICATION or ULTRASONICATION. Sonicators commonly work
on the principle of magnetostriction: the resonant deformation
exhibited by certain types of metal in an alternating magnetic
718
SOS system
SOS system A system in which the expression of certain genes
(SOS genes) is induced (turned on, or enhanced) in response
to damaged DNA or to inhibition of DNA replication caused
e.g. by the effects of ULTRAVIOLET RADIATION or the action of
an ALKYLATING AGENT or quinolone antibiotic (such as NALIDIXIC
ACID). (The SOS system can also be induced e.g. by the CcdB
toxin: an agent, encoded by the F plasmid, which affects gyrase
at sites other than those targeted by the quinolone antibiotics
[TIM (1998) 6 269275].)
The SOS response results in e.g. inhibition of cell division,
an increased capacity for DNA repair, alleviation of restriction,
an altered pattern of energy metabolism, and (in those strains
which contain a COLICIN PLASMID) production of colicin; it also
gives rise to an increased rate of mutation.
The SOS system has been studied mainly in Escherichia coli,
and the following account refers primarily to the operation of
the SOS system in that organism.
Control of the SOS response. The SOS system consists of
about 30 unlinked genes which are normally repressed by the
LexA protein (lexA gene product). LexA (perhaps as a dimer)
inhibits transcription by binding to an operator sequence (an
SOS box ) in the promoter region of each gene or operon; the
binding site for LexA is apparently the consensus sequence
5 -CTGTN8 ACAG-3 (in which N8 is an 8-nucleotide sequence).
Different SOS boxes have different levels of affinity for LexA,
and many of the SOS genes are expressed at low levels even in
the repressed state. (At least one SOS gene, uvrB, has a second
promoter which is not subject to control by LexA.) The LexA
protein also represses its own synthesis; however, the SOS box
of the lexA gene has a low affinity for LexA, so that there is
always enough LexA to repress the other SOS genes.
Damaged DNA activates the RECA PROTEIN in an unknown
way, i.e. the precise nature of the SOS-inducing signal is not
known although it is generally believed to involve a region of
ssDNA and/or product(s) of DNA degradation.
Activated RecA (designated RecA ) behaves as a CO-PROTEASE
which triggers the autocatalytic cleavage of LexA permitting
expression of the SOS genes. In vitro studies on the cleavage of
LexA have suggested that cleavage occurs more rapidly when a
chi (c) site (5 -GCTGGTGG-3 ) occurs near a double-stranded
break in DNA; it may be that the presence of c promotes
activation of RecA [Cell (1998) 95 975979].
Weak SOS-inducing signals (due e.g. to low-level damage to
DNA) may lower the intracellular concentration of LexA to only
a limited extent so that only those SOS genes with low-affinity
SOS boxes will be induced.
Inhibition of cell division. One aspect of the SOS response
is a temporary inhibition of septum formation (and, hence, cell
division); mutants in which the SOS system is constitutively
de-repressed form aseptate filaments.
During induction of the SOS system, septum formation is
prevented as a result of inhibition of polymerization of the FtsZ
protein (product of the ftsZ gene: see Z ring in CELL CYCLE
(b)). Polymerization of FtsZ is blocked by SulA, product of the
SOS gene sulA (= sfiA) [JB (1998) 180 39463953]; cells may
continue to grow as septum-less filaments. (Previously, some
mutant alleles of ftsZ were referred to as sulB and sfiB.)
SulA is normally very unstable, so that when repression of
sulA is re-imposed normal septation is rapidly restored. At least
part of the instability of SulA is due to its proteolytic inactivation by the product of the lon gene; in lon mutants SulA is
much more stable, and induction of the SOS response even
by mild ultraviolet radiation may lead to lethal filamentation.
souma
(Lon is a HEAT-SHOCK PROTEIN; note that the heat-shock response
can be triggered by certain factors such as ultraviolet radiation which induce the SOS system.)
A temporary inhibition of cell division may be advantageous
to the cell in that the cell is given time to carry out repairs to
damaged DNA.
DNA repair. The UvrABC-dependent nucleotide excision
repair system (including genes uvrA and uvrB ) and the RECOMBINATION REPAIR system are enhanced in the SOS response; these
repair systems have a high degree of accuracy (error-free
repair).
Another repair system, which is apparently expressed only
when the SOS system is induced, involves genes umuC and
umuD; the operation of this so-called error-prone repair system (also called mutagenic repair) results in an increased rate
of mutation (which is referred to as SOS mutagenesis). In this
process, RecA , acting as a co-protease, mediates autocatalytic
cleavage of UmuD to an active fragment, UmuD (see DNA POLYMERASE V). SOS mutagenesis is believed to involve DNA (repair)
synthesis on a template strand that contains a lesion e.g.
a pyrimidine dimer (two adjacent, covalently linked pyrimidines on the same strand); such translesion synthesis is likely
to involve specific DNA polymerase(s) induced as part of the
SOS response including DNA POLYMERASE V, DNA POLYMERASE
IV and DNA polymerase II (polB gene product) [TIBS (2000) 25
7479]. Because of a local loss of base-pairing specificity at the
lesion, repair synthesis is likely to introduce incorrect bases and
give rise to a mutant genome. (See also WEIGLE REACTIVATION.)
Once the damaged DNA has been repaired, RecA becomes
inactive as a co-protease; as the lexA gene is induced during
the SOS response, the high level of LexA being synthesized
means that, when activated RecA disappears, repression of the
SOS genes (and restoration of normal cell function) can occur
rapidly.
Systems resembling the SOS system in E. coli have been
observed in some other Gram-negative bacteria e.g. species of
Bacteroides, Rhizobium and Salmonella as well as in Bacillus
subtilis (SOB system).
Many bacteria appear to be inherently resistant to mutagenesis induced by ultraviolet radiation, and seem not to possess a
umuDC function; such bacteria include Deinococcus radiodurans, Haemophilus influenzae, Proteus mirabilis, Streptococcus
pneumoniae and Salmonella typhimurium.
Functional homologues of umuC and umuD are carried by
certain conjugative plasmids (e.g. ColI, R46 and its derivative
pKM101, R205); the genes mucA and mucB in pKM101 are
able to suppress the non-mutability of E. coli umuC and umuD
mutants, and when introduced into cells which normally lack
a umuCD system, pKM101 can decrease the susceptibility of
those cells to killing while increasing their susceptibility to
mutagenesis on exposure to umuCD-dependent mutagens. (See
also AMES TEST.) [Plasmid genes affecting DNA repair and
mutation: JCS (1987) 6 (supplement) 303321.]
The SOS system may be viewed as an adaptive genetic
response to specific types of unfavourable environment. Under
these conditions it is advantageous for bacteria to be able to
make essential repairs and to adapt rapidly by making use of any
(fortuitous) new combinations of nucleotides that may enhance
their survival. This is reflected in increased repair activity and
also in SOS mutagenesis the latter offering the possibility of
beneficial as well as lethal mutations. Suppression of restriction
may favour exploitation of imported DNA, while inhibition of
cell division may help e.g. to conserve energy and avoid the
formation of non-viable daughter cells.
Error-prone repair in in vitro mutagenesis. A variety of mutagenic agents depend on the umuDC system for their mutagenic
effects; thus, umuDC mutants of E. coli are resistant to the
mutagenic effects of e.g. ultraviolet radiation and methylmethane
sulphonate (see ALKYLATING AGENTS) but can still be mutated
by agents such as MNNG and ethylmethane sulphonate (see ALKYLATING AGENTS) which cause lesions leading directly to base
mispairing.
souma NAGANA caused (usually or exclusively) by Trypanosoma
vivax.
sour cream Cultured sour cream is made by the fermentation of
pasteurized and homogenized cream (1820% milk fat) using
the same organisms as for BUTTERMILK.
sourdough bread See BREAD-MAKING.
South American blastomycosis Syn. PARACOCIDIOIDOMYCOSIS.
Southampton virus See SMALL ROUND STRUCTURED VIRUSES.
Southern bacterial wilt Syn. GRANVILLE WILT.
southern bean mosaic virus See SOBEMOVIRUSES.
Southern blot (Southern blotting) (1) A BLOTTING technique in
which DNA is transferred from a gel to a nitrocellulose matrix
(see figure).
(2) Erroneously, a synonym of SOUTHERN HYBRIDIZATION.
Southern hybridization A procedure used e.g. to detect a
specific sequence of nucleotides among fragments of DNA
which have been separated by gel electrophoresis. Initially,
using the SOUTHERN BLOT technique (q.v.), single-stranded forms
of the fragments are bound to a matrix. In the next step
(Southern hybridization) the matrix is exposed to a labelled
PROBE complementary to the sequence of interest; HYBRIDIZATION
(sense 1) between the probe and a specific region of the blotted
DNA (detected by the probes label) indicates the required
sequence.
Southwestern blotting A technique for detecting DNA-binding
proteins in a cell lysate etc. The sample is initially subjected
to gel electrophoresis, and the proteins thus separated are
electroblotted (see BLOTTING) onto a nitrocellulose filter. The
affinity of any blotted protein for a specific DNA sequence is
then determined by using labelled DNA sequences as probes
and detecting the label of any probe which has bound to a given
protein.
soy paste Syn. MISO.
soy sauce (shoyu) A condiment traditionally prepared by fermenting soybeans and (usually) wheat (cf. TAMARI SAUCE). A
KOJI (made from whole or defatted soybeans and crushed roasted
wheat) is transferred to a deep vessel and is suspended in brine
(to 1719% NaCl) to form moromi; the moromi is allowed
to ferment, usually with occasional agitation and aeration, for
e.g. 68 months or more. During this stage, enzymes from the
koji mould hydrolyse proteins and starch in the raw materials
to provide low-MWt substrates which are initially fermented
primarily by lactic acid bacteria (e.g. Lactobacillus delbrueckii,
Pediococcus halophilus); the pH falls rapidly to ca. 5.0 or lower,
after which fermentation is continued primarily by yeasts (e.g.
Zygosaccharomyces rouxii ). Torulopsis spp (Candida etchellsii, C. versatilis) may grow at later stages in the fermentation;
these yeasts produce substances which contribute to the flavour
and aroma of the final product. The soy sauce fermentation may
be carried out by microorganisms naturally present in the raw
materials, or pure cultures of selected strains may be used. After
the fermentation, the raw soy sauce is decanted or pressed from
the solid residue and is pasteurized, filtered and bottled. [Book
ref. 5, pp. 3986; microbes used in soy sauce manufacture: Food
Mic. (1984) 1 339347.]
720
species
weight
nitrocellulose
paper towels
gel
wick
SOUTHERN BLOT (Southern blotting): the transfer of DNA fragments from a gel strip to a sheet of nitrocellulose by capillary action.
Within the gel, the fragments are distributed in discrete zones, according to size, having been previously separated by gel electrophoresis.
The fragments are first denatured (made single-stranded) by exposing the gel to alkali; the gel is then exposed to neutral buffer and arranged
as shown in the diagram. Driven by capillary action, the neutral, saline solution in the dish rises, via the wick, into and through the gel, through
the (permeable) nitrocellulose, and into the stack of paper towels; this upward stream of liquid carries the DNA fragments from the gel to the
sheet of nitrocellulose. Importantly, the relative positions of fragments on the sheet are the same as they were in the gel. The sheet is removed
and baked at 70 C under vacuum to bind the DNA. The fragments can then be examined e.g. by exposing the sheet to a specific labelled
probe; probetarget binding (= Southern hybridization), detected by the probes label, identifies the required sequence.
One alternative to nitrocellulose is APT PAPER (q.v.). This not only avoids the need for baking, it also permits removal of probes so that
different probes can be subsequently used on the same sheet.
Northern blotting refers to the transfer of RNA from gel to matrix.
Western blotting refers to the transfer of protein from gel to matrix.
Electroblotting is a faster method which uses an electric field for effecting transfer.
Figure reproduced from Bacteria 5th edition, Figure 8.13, page 195, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN
0471-98880-4) with permission from the publisher.
or intracellular stroma. Ascocarp: perithecioid. Asci: unitunicate, deliquescent. Ascospores: appendaged, some spoon-shaped
(spathulate). The sole genus, Spathulospora, is classified in the
LABOULBENIALES by some authors.
spawn (mycol.) Mycelium usually of Agaricus brunnescens (A.
bisporus) growing e.g. in a block (brick) of horse manure,
used as an inoculum in MUSHROOM CULTIVATION. It may be
derived from a previous culture or may be grown by inoculating
sterile compost with spores of a selected strain.
spc operon In e.g. Escherichia coli: an OPERON containing genes
for r-proteins L14, L24, L5, S14, S8, L6, L18, S5, L30, and L15,
and gene prlA (= secY: involved in protein secretion), listed in
order of transcription. (See RIBOSOME.)
SpeI See RESTRICTION ENDONUCLEASE (table).
speB gene (Streptococcus) See NECROTIZING FASCIITIS.
special form Syn. FORMA SPECIALIS.
specialized transduction See TRANSDUCTION.
speciation (1) The evolutionary process which leads to the
formation of new species. (2) The taxonomic process by which
species are delimited.
species (microbiol.) (singular and plural: species) One of the
less-inclusive categories in TAXONOMY the individuals of a
given species displaying a high degree of mutual similarity; a
universally applicable and acceptable definition of species is
currently not available.
Among microorganisms, SPECIATION (sense 2) was particularly
unsatisfactory for prokaryotes prior to the mid-1960s. Since
then, molecular methods have progressively provided a basis for
what is thought to be a PHYLOGENETIC CLASSIFICATION of these
organisms. Such methods include DNA HOMOLOGY studies and the
comparison of organisms on the basis of nucleotide sequences
in their 16S rRNA.
721
species nova
spermatiophore A modified or undifferentiated hypha which
bears a SPERMATIUM.
spermatium A non-motile male reproductive cell which can
function in SPERMATIZATION. (cf. MICROCONIDIUM (sense 1) and
PYCNIOSPORE.)
spermatization In certain higher fungi: the union of a SPERMATIUM with a female reproductive structure (e.g. a TRICHOGYNE
or a FLEXUOUS HYPHA).
spermatogonium Syn. SPERMAGONIUM.
spermidine See POLYAMINES.
spermine See POLYAMINES.
spermogonium Syn. SPERMAGONIUM.
Spermophthora See METSCHNIKOWIACEAE.
Spermophthoraceae Syn. METSCHNIKOWIACEAE.
SPF SPECIFIC PATHOGEN FREE.
SPf66 vaccine See MALARIA.
Sphacelaria See PHAEOPHYTA.
Sphacelia A genus of fungi of the HYPHOMYCETES; teleomorphs
occur e.g. in the genus CLAVICEPS.
Sphaceloma
A genus of fungi of the COELOMYCETES. Teleomorph: Elsinoe.
Sphacelotheca See USTILAGINALES.
Sphaeractinomyxon See ACTINOSPOREA.
Sphaeriales An order of fungi (subdivision ASCOMYCOTINA)
which typically form carbonaceous perithecia (often containing filiform paraphyses) immersed in a stroma. Asci: unitunicate, cylindrical or ellipsoidal. Ascospores: aseptate or septate,
colourless or dark. Genera: e.g. Ascotricha, Camarops, DALDINIA,
Hypoxylon, XYLARIA.
Sphaerobolus A genus of lignicolous and coprophilous fungi
(order SCLERODERMATALES) formerly classified in the Nidulariales. S. stellatus forms globose basidiocarps (ca. 1.52.5 mm
diam.) in which the peridium is composed of six layers. At maturity, the glebal mass is violently discharged following rupture of
the peridium and the sudden eversion of certain inner layers;
eversion occurs apparently as a result of increased osmotic pressure in one of the inner layers (due to the breakdown of glycogen
to soluble sugars) and the consequent stress upon this (and an
adjacent) layer on absorption of water. [Culturing for fruiting
bodies: Mycol. (1984) 76 944946.]
sphaerocyst A spherical or ovoid cell, numbers of which occur
in the TRAMA, and in other parts of the CONTEXT, e.g. in fungi of
the genera Lactarius and Russula.
sphaerocyte An (abnormal) spherical or subspherical form of an
erythrocyte formed, e.g., as a result of the activity of Escherichia
coli a-haemolysin.
Sphaerocytophaga
A genus of bacteria; the organisms are
similar or identical to species of CAPNOCYTOPHAGA [Book ref. 45,
pp. 356379 (365)].
Sphaerodes See SORDARIALES.
Sphaerodothis See POLYSTIGMATALES.
sphaeromastigote A form assumed by the cells of species of
Trypanosoma during certain stages of their life cycles: see
TRYPANOSOMATIDAE.
Sphaeromonas A genus of fungi found in the RUMEN.
Sphaeromyxa See MYXOSPOREA.
Sphaerophoraceae See CALICIALES.
Sphaerophorus (1) (mycol.) See CALICIALES. (2) (bacteriol.) Obsolete genus of bacteria which are currently included in the
genera BACTEROIDES and FUSOBACTERIUM.
Sphaerophrya See SUCTORIA.
sphaeroplast (spheroplast) A spherical or near-spherical, osmotically sensitive structure which resembles a PROTOPLAST but is
Spirillospora
group at C-2 of sphingosine forms an amide bond with a longchain fatty acid (forming ceramide), and the terminal (C-1)
hydroxyl is esterified with phosphorylcholine.
sphingomyelinase A PHOSPHOLIPASE (q.v.) which cleaves SPHINGOMYELIN. An example is the staphylococcal b-HAEMOLYSIN, a
C-type phospholipase which cleaves sphingomyelin to phosphorylcholine and ceramide. (See also HOTCOLD LYSIS.) Corynebacterium pseudotuberculosis (formerly C. ovis) forms a sphingomyelinase (a D-type phospholipase) which cleaves choline
from sphingomyelin.
sphingosine See SPHINGOLIPID.
SPI Salmonella PATHOGENICITY ISLAND.
spiculum A narrow, apical extension of a STERIGMA on which a
spore is borne.
spin killing A type of killing of sensitive strains of Paramecium
by certain types of killer paramecia (e.g. strains containing
Caedibacter varicaedens); affected cells swim with rapidly
reversing rotational movements.
spin label See ELECTRON SPIN RESONANCE.
spina (pl. spinae) In certain prokaryotes (e.g. some pseudomonads): a hollow, rigid, apparently non-prosthecate appendage, one
or more of which project from the cell surface; it is a thin-walled
structure formed from a cross-linked helical filament. [Conical
spinae: CJM (1984) 30 716718. Possible function: JGM (1991)
137 10811086.]
spinach latent virus See ILARVIRUSES.
spindle (1) See MITOSIS and MEIOSIS. (2) (virol.) See ENTOMOPOXVIRINAE.
spindle pole body (syn. centriolar plaque; polar plaque) In some
types of eukaryotic cell (including e.g. Saccharomyces cerevisiae):
a body which is embedded in the nuclear membrane and
which can act e.g. as a MICROTUBULE-ORGANIZING CENTRE during
MITOSIS.
spinning disease A FISH DISEASE which affects the Atlantic
menhaden (Brevoortia tyrannus); the disease tends to occur in
large-scale annual epizootics with massive mortalities. Terminal
symptoms include loss of coordination and erratic swimming
behaviour. The causal agent is a virus which closely resembles
(and may be identical to) IPN VIRUS.
spinoculation Centrifugally-assisted enhancement of transduction efficiency (a procedure in which the virus vector and cells
are centrifuged together).
spira Refers to helical aerial hyphae one of three categories
used in a system for the morphological classification of streptomycetes; the other two categories are rectusflexibilis (straight
to flexuous hyphae) and retinaculum apertum (hook-shaped,
looped, or spiral hyphae with one or two turns). [Disadvantages
of the system: Book ref. 46, p. 2067.]
spiral plate count method A method used for counting bacteria
in samples of milk. Essentially, the inoculum is delivered from a
syringe onto a rotating plate so that it is deposited along a spiral
path; the volume of inoculum delivered to a particular region of
the plate can be read off from the apparatus. A colony count is
made after incubation of the plate.
spiramycins See MACROLIDE ANTIBIOTICS.
Spirillaceae A family of bacteria which formerly included the
genera Campylobacter and Spirillum but which has been abandoned pending further taxonomic studies [Book ref. 22, p. 71].
Spirillospora A genus of bacteria (order ACTINOMYCETALES, wall
type III; group: maduromycetes) which occur e.g. in soil and
leaf litter. The organisms form thin (<1 m diam.) branching
substrate and aerial mycelium, the latter giving rise to spherical
sporangia (up to ca. 24 m diam.); in water, mature sporangia
spirilloxanthins
release motile (flagellated) rod-shaped spores. Type species:
S. albida. [Book ref. 73, p. 113.]
spirilloxanthins See CAROTENOIDS.
spirillum (1) Any spiral-shaped, relatively rigid bacterial cell.
(2) Any species or strain of Spirillum.
Spirillum
A genus of Gram-negative, asporogenous bacteria. Cells: rigid, helical, ca. 1.41.7 1460 m. POLAR MEMBRANES and PHB granules are formed, COCCOID BODIES are
not. Motile: bipolar tufts of flagella of long wavelength.
Microaerophilic. Metabolism is respiratory; nitrate respiration
does not occur. Oxidase +ve; catalase ve; phosphatase +ve;
indole ve; arylsulphatase ve. Growth is inhibited by NaCl
levels >0.02%, and by phosphate >0.01 M. Carbohydrates are
not utilized; carbon sources: salts of organic acids (e.g. succinate). GC%: 38. Type species: S. volutans, found in stagnant freshwater habitats. (cf. AQUASPIRILLUM; AZOSPIRILLUM;
OCEANOSPIRILLUM; SPOROSPIRILLUM.)
Species incertae sedis: S. minus (= S. minor ), causal agent
of one form of RAT-BITE FEVER; cells: ca. 0.2 35 m, usually
spiral, actively motile by one or more flagella at each pole.
S. pulli, apparent causal agent of DIPHTHEROID STOMATITIS in
chickens; cells: rigid spirals, ca. 1.0 512 m, motile with
one flagellum at each pole.
[Book ref. 22, pp. 9093. Culture, media etc: Book ref. 45,
pp. 597599.]
spirits Alcoholic beverages prepared by the distillation of fermented liquors or mashes. The characteristic flavours and qualities of the various spirits are determined by the nature of the
fermented raw materials, conditions of distillation, effects of
ageing, etc. The fermentation stage generally resembles that in
BREWING or WINE-MAKING. Use is made of yeast (Saccharomyces)
strains which effect maximum attenuation (i.e. they convert the
maximum amount of carbohydrate to alcohol); these strains are
characterized by high alcohol-tolerance. Distillers yeasts produce a range of higher alcohols (FUSEL OIL) which contribute to
the aroma and flavour of the product. Spirits are not subject to
microbial spoilage owing to their high alcohol content.
Bourbon is an American whisky (whiskey) made by distilling
a fermented mash containing maize and rye. Brandy (cognac)
is prepared by distilling grape wine. Gin is made by distilling
fermented rye or maize worts and redistilling the product in a
still containing herbs and juniper berries (botanicals). Rum is a
distillate of fermented molasses or sugarcane products. Tequila:
see PULQUE. Whisky is distilled either from a wort derived from
malted barley (malt whisky) or from a mash of unmalted grain
(often barley or maize) mixed with a proportion of malted barley
(grain whisky).
Spirochaeta
A genus of Gram-negative bacteria of the family SPIROCHAETACEAE; the organisms, which include both obligately and facultatively anaerobic species, occur as free-living
inhabitants of freshwater and marine environments, including
muds, and are common in H2 S-containing habitats. The cells
are 0.20.75 5250 m; the type species, S. plicatilis, contains many periplasmic flagella per cell, but the other species
contain only two per cell. The organisms are motile in liquids and can also creep over solid surfaces and migrate through
agar (1%) the latter feature being useful in isolation procedures. In most species the anaerobic metabolism of carbohydrates yields ethanol, acetate, CO2 and H2 ; S. zuelzerae forms
lactate and succinate. GC%: ca. 5165.
Species differentiation is based on e.g. cell diameter, ability
to grow aerobically, NaCl requirement and pigmentation. Six
species are recognized [Book ref. 22, pp. 3946]: S. aurantia
split gene
contain DNA; they may belong in the INOVIRIDAE. In SV-C2
phages there is an icosahedral-type head (5258 4851 nm)
with a tail (7583 68 nm) attached at one vertex. SVC3 phages (= C3 strain C3 phages) probably belong to the
PODOVIRIDAE; the icosahedral-type head (ca. 40 3537 nm)
contains linear dsDNA (MWt 1.4 107 ) and has a short tail
(1318 68 nm) attached at one vertex. SV-C3 progeny
virions seem to be released in host-derived membrane vesicles.
(See also MYCOPLASMAVIRUSES).
Spirosoma A genus of yellow-pigmented bacteria (family SPIROSOMACEAE). The cells, 0.51.0 1.56.0 m, are commonly
helical or curved rods ring-shaped forms sometimes being
seen as a result of overlap of the ends of highly curved cells.
Acid is formed from many carbohydrates. GC%: 5153. Type
species: S. linguale.
Spirosomaceae A family of Gram-negative, obligately aerobic,
chemoorganotrophic, pink- or yellow-pigmented bacteria which
occur in soil and aquatic habitats; the organisms are rigid,
straight, curved or spiral, non-motile rods. Growth (optimum
temperature range: 2030 C) occurs e.g. on peptoneyeast
extractglucose agar. Genera: FLECTOBACILLUS, RUNELLA, SPIROSOMA. [Book ref. 22, pp. 125132.]
Spirostomum A genus of ciliate protozoa (order HETEROTRICHIDA)
which occur e.g. in microaerobic freshwater and estuarine
habitats. Cells: elongate, cylindrical, up to ca. 4 mm in
length but able to contract to a fraction of their normal length;
somatic ciliature is uniform, and the cytostome is lateral. A large
posterior contractile vacuole discharges via a long canal which
opens to the exterior near the anterior end. In some species (e.g.
S. ambiguum) the macronucleus is moniliform, in others (e.g.
S. teres) it is ovoid.
spirotrich A member of the Spirotrichia.
Spirotrichia See POLYHYMENOPHOREA.
Spirotrichonympha See HYPERMASTIGIDA.
Spirulina A genus of filamentous CYANOBACTERIA (section III)
in which the trichomes are helical with little or no constriction
between adjacent cells. GC%: 4453. The trichomes show
GLIDING MOTILITY, and the tips are capable of a twitching or
jerking motion which may be brought about by a contractile
(actin-like?) protein [Book ref. 76, pp. 420421]. Spirulina
typically occurs in warm, saline, alkaline lakes, where it forms
dense tangled masses. For centuries it has been used as food by
people in the Lake Chad region of Africa, and was also eaten by
the Aztecs of ancient Mexico; in Africa, the masses of growth
are collected, sun-dried, and made into thin cakes which may be
eaten directly or after cooking.
Spitzenkorper (apical granule) A small, densely staining body
which occurs, close to the cytoplasmic membrane, in the tip
of an actively growing fungal hypha; in at least some fungi it
consists of a cluster of vesicles associated with microfilaments.
(See also GROWTH (fungal).)
spleen focus-forming virus (SFFV) See FRIEND VIRUS and RAUSCHER VIRUS.
splenic fever See ANTHRAX.
splice sites See SPLIT GENE.
spliceosome See SPLIT GENE (a).
splicing (1) (of RNA) See SPLIT GENE. (2) (of DNA) See e.g.
CLONING.
split gene (interrupted gene) A structural gene (encoding e.g. a
protein, rRNA or tRNA) that contains one, several or many specific sequences of nucleotides (intervening sequences; introns)
which, although represented in the primary RNA transcript of
the gene, are absent from the mature RNA molecule (mRNA,
split gene
initially involves cleavage at the 5 splice site, thus releasing
the 3 end of the 5 exon, and formation of an intron3 -exon
intermediate in the form of a lariat (a tailed, circular molecule);
the lariat results from the formation of a 2 5 phosphodiester
bond between the (free) 5 end of the intron and a site within the
intron near its 3 end (the branch point). In yeast, this branch
occurs at the last adenine residue in the TACTAAC box.
Subsequently, the 3 splice site is cleaved, and the 5 and 3
exons are ligated. The intron, released as a lariat, is debranched,
enzymically, to release a free linear intron (which is degraded in
vivo). Debranching enzymes from S. cerevisiae and Schizosaccharomyces pombe exhibit some homology with the human RNA
lariat debranching enzyme [NAR (2000) 28 36663673].
Secondary or tertiary structure in the intron appears not to be
important for the juxtaposition of splicing sites in nuclear introns
(cf. other mechanisms below).
The splicing reaction depends on certain small molecules of
RNA snRNAs (see SNRNA) which apparently act as external
guide sequences (EGSs) to locate the relevant sites in the premRNA. In higher eukaryotes, U1 snRNP binds to the 5 splice
site (the 5 end of U1 snRNA probably base-pairing with the
conserved sequence GUNAGU), U2 snRNP binds to the branch
point, and U5 snRNP probably binds to the 3 splice site.
Interactions between the snRNPs, and between snRNPs and
the RNA substrate, presumably bring about juxtaposition of the
3 and 5 splice sites. Splicing of the pre-mRNAs in yeasts and in
higher eukaryotes involves a large (40S60S) ribonucleoprotein
particle (the spliceosome) which, in e.g. human cells, contains
U snRNPs; in yeasts, the spliceosome contains at least three
snRNAs, and its assembly is dependent on the presence of a 5
splice site and a TACTAAC box within the RNA [Cell (1986)
45 869877].
(b) Group I introns (= class I introns). Introns of this type
occur in nuclear pre-rRNA of Tetrahymena thermophila and
Physarum polycephalum, in several fungal mitochondrial prerRNAs and pre-mRNAs, and in certain chloroplast tRNA genes.
They are characterized by a common splicing mechanism and
by a number of conserved sequences; interaction between these
sequences apparently folds the intron into a core structure in
which the 5 and 3 splice sites are brought into close proximity.
Excision of this type of intron is an intrinsic property of the
RNA itself, i.e. group I introns are self-splicing or autocatalytic;
in some cases splicing can occur in vitro when the RNA is
incubated with divalent cations and guanosine or a guanosine
nucleotide (GMP, GDP or GTP or a G at the 3 end of
an oligo- or polynucleotide) in the absence of protein. (cf.
RIBOZYME.)
Splicing involves two distinct and independent cleavageligation steps and transesterification reactions in which
the total number of phosphodiester bonds remains constant (so
that splicing does not require an additional source of energy).
Cleavage occurs first at the 5 splice site concomitantly with
the formation of a phosphodiester bond between the 3 -OH of
a guanine nucleoside or nucleotide and the 5 end of the intron.
Subsequently, cleavage of the 3 splice site is coupled with
ligation of the 5 and 3 exons. In many cases the excised linear
intron circularizes by a transesterification reaction in which
the 3 -terminal residue (usually or always a guanosine residue)
forms a covalent bond at a site near the 5 end, the terminal
oligonucleotide being released.
It has been proposed that, during the splicing process, a
nucleotide sequence within the 5 exon (adjacent to the 5 splice
site) base-pairs with a complementary sequence within the intron
tRNA etc.) and, hence, do not encode any part of the gene product. Thus, maturation of the primary RNA transcript of a split
gene must involve a process of splicing in which sequence(s)
corresponding to intron(s) are deleted (spliced out) and the
remaining sequences (termed exons) are joined together; for
example, in the case of mRNA (q.v.), the amalgamated exons
form the complete coding sequence of the gene together with
any non-coding leader and/or trailer sequences.
In some cases a given gene can be spliced in different ways
to yield different versions of the encoded product, i.e. splicing
can give rise to different combinations of exons producing
correspondingly different coding sequences. Such alternative
splicing can be advantageous to a cell e.g. in that synthesis
of multiple products from a single gene permits economy in the
size of the genome.
Introns are often non-coding sequences that are degraded
following excision but see (b) and (c), below, and INTRON
HOMING.
Split genes occur in eukaryotes and in certain prokaryotes
(including bacteria and archaeans) and viruses. Many (or most)
eukaryotic genes contain at least one intron sometimes many;
the gene encoding type I collagen appears to contain about 50
introns. By contrast, the (human) insulin gene contains only one
intron, while the gene encoding interferon-b is intron-less.
In higher eukaryotes, many (perhaps most) of the nuclear
structural genes are split genes, but in typical eukaryotic
microorganisms (e.g. Dictyostelium, Saccharomyces) fewer of
these genes are reported to contain introns, and the introns tend
to be smaller than those in higher eukaryotes; by contrast, no
intron-less protein-encoding genomic sequences were seen in the
database of Physarum polycephalum each gene containing, on
average, 3.7 introns [NAR (2000) 28 34113416].
Splicing of the RNA transcript of a split gene involves
cleavage of a precise phosphodiester bond at both ends of each
intron (at the exonintron junctions) the 5 and 3 splice sites;
this is followed by the formation of a phosphodiester bond
between the exon at the 5 end of the intron (the 5 exon) and
the exon at the 3 end (the 3 exon). Details of the splicing
mechanism differ in different types of split gene.
Split genes in eukaryotes are considered in (a) to (d), below;
split genes in prokaryotes and viruses are considered in (e).
(a) Nuclear mRNA introns. In nuclear protein-encoding genes
of e.g. Saccharomyces cerevisiae, the introns have been found
to contain three CONSENSUS SEQUENCES that are necessary for
splicing:
GTATGT
at the 5 end of the intron,
PyAG
at the 3 end, and
TACTAAC
(the TACTAAC box) near the 3 end. These sequences are
those in the DNA strand which has the same sequence as the
RNA transcript; they may also be written in terms of the RNA
itself, e.g. TACTAAC = UACUAAC.
The consensus sequences mentioned above may differ somewhat in other eukaryotes, but nearly all introns of this type have
the 5 terminal GT (the 5 , left or donor splice site) and the
3 -terminal AG (the 3 , right or acceptor splice site); this is the
so-called GT. . .AG (or GU. . . AG) rule.
Excision of an intron from a pre-mRNA molecule (transcribed
by RNA polymerase II) depends on trans-acting factors and
726
spoligotyping
transcript. Thus, the very long polycistronic viral RNA transcripts produced in these cells can be spliced in different
ways generating functional mRNAs in which the same 5 cap
and leader sequence is spliced onto different coding sequences.
(See also SUBGENOMIC MRNA.) Certain small adenovirus-encoded
RNAs (the VA RNAs) which associate with cellular proteins forming RNP particles may be involved in splicing
viral RNA; VA1 RNA is apparently complementary to splicing
junctions in some adenovirus genes.
Among archaeans, some tRNA genes contain an intron which,
when transcribed, gives rise to a corresponding sequence within
the anticodon arm of the pre-tRNA molecule; the position of
the intron is generally similar to that in yeast tRNA genes (i.e.
on the 3 side of the anticodon), but in the extreme thermophile
Thermoproteus tenax a tRNALeu contains an intron within the
anticodon sequence itself, while tRNAAla has an intron in a
unique position on the 5 side of the anticodon in the stem of
the anticodon arm [EMBO (1987) 6 523528].
Bacterial introns appear to be mainly or solely of the autocatalytic type (group I or group II). The bacterial group I introns
seem to occur primarily within tRNA genes; they have been
found e.g. in the purple bacterium Azoarcus and the cyanobacterium Synechococcus [structurefunction relationships of the
intron ribozymes of Azoarcus and Synechococcus: NAR (2000)
28 32693277], in Anabaena and other cyanobacteria, in
Agrobacterium tumefaciens and in Simkania negevensis (a member of the Chlamydiales in which the intron interrupts a 23S
rRNA gene).
Bacterial group II introns (like group I introns) are mobile
genetic elements but are not primarily associated with tRNA
genes. Group II inrons have been found e.g. in Lactococcus
spp and in Escherichia coli, Pseudomonas alcaligenes and
Streptococcus pneumoniae. [Bacterial group II introns (review):
Mol. Microbiol. (2000) 38 917926.]
In some cases, splicing in bacteria may occur while the
transcript is still bound to a ribosome [splicing and translation
in bacteria (perspective): GD (1998) 12 12431247]. Splicing
in vivo has been demonstrated for a group II intron in the
conjugative transposon Tn5397 [JB (2001) 183 12961299].
Bacterial introns (of both groups I and II) can propagate by
INTRON HOMING. [Barriers to intron promiscuity in bacteria: JB
(2000) 182 52815289.]
split-product vaccine (split-virus vaccine) A VACCINE which
contains some of the components of a virus (as opposed to whole
virions).
split-virus vaccine See SPLIT-PRODUCT VACCINE.
splitter See TAXONOMY.
spo mutant See ENDOSPORE (sense 1(a)).
Spo0AP See ENDOSPORE (sense 1).
Spo0E See ENDOSPORE (sense 1).
Spo0F See ENDOSPORE (sense 1).
SpoIIB See ENDOSPORE (figure (a) legend).
SpoIID See ENDOSPORE (figure (a) legend).
spoIIG See ENDOSPORE (figure (a) legend).
SpoIIM See ENDOSPORE (figure (a) legend).
SpoIIP See ENDOSPORE (figure (a) legend).
SpoIIIE See ENDOSPORE (figure (a) legend).
spoilage See BIODETERIORATION.
spoligotyping A rapid, PCR-based method for simultaneously
detecting and typing strains of the Mycobacterium tuberculosis complex [original description: JCM (1997) 35 907914].
Essentially, PCR is used to amplify spacer sequences in the
direct repeat (DR) locus of the chromosome (which apparently
Spondweni virus
24
3
DR
25
DR
26
DR
DR
M. tuberculosis H37Rv
negative control
1
2
3
4
5
6
7
8
9
spore ball
basipetally formed chains; in many fungi (e.g. Mucor ) the sporangium contains a COLUMELLA. A sporangium may be deciduous
at maturity (e.g. in Dictyuchus) or it may remain attached to
the sporangiophore (e.g. in Saprolegnia); the spores may be
released via a pore or by dissolution of the sporangial wall. In
e.g. Pilobolus the entire sporangium is forcibly discharged. (See
also meiosporangium and mitosporangium under ALLOMYCES,
and zygosporangium under ZYGOSPORE.)
(2) (bacteriol.) The cell in which an ENDOSPORE is formed.
(3) (bacteriol.) That part of a cell which subsequently develops into an endospore.
(4) (bacteriol.) In e.g. Actinoplanes and members of the
MYXOBACTERALES: a specialized structure containing one or more
spores.
spore A differentiated form of an organism which may be (a)
specialized for dissemination; (b) produced in response to, and
characteristically resistant to, adverse environmental conditions;
and/or (c) produced during or as a result of an asexual or sexual
reproductive process. (Not all microorganisms can produce
spores.) A spore may be unicellular (i.e., it may contain only one
protoplast), bicellular, or multicellular; it may be thick-walled
or thin-walled, pigmented or non-pigmented, motile or nonmotile. Under suitable conditions, disseminative and resistant
forms of spore typically give rise to a vegetative organism(s); a
spore formed in a reproductive process may e.g. give rise to a
vegetative organism or act as a gamete.
Bacterial spores. Bacterial ENDOSPORES (q.v.) are resistant
(and may be disseminative) forms rather than reproductive
forms, while the EXOSPORES formed e.g. by species of the ACTINOMYCETALES (q.v.) are characteristically reproductive and disseminative forms. (See also myxospores in MYXOBACTERALES.)
Fungal spores. See e.g. ASCOSPORE; AZYGOSPORE; BALLISTOSPORE; BASIDIOSPORE; CHLAMYDOSPORE; CONIDIUM (and SACCARDOAN SYSTEM); GEMMA; OIDIUM; SPORANGIOSPORE; STATISMOSPORE; THALLOSPORE; ZYGOSPORE. (See also UREDINIOMYCETES
and USTILAGINALES.)
Some fungal spores exhibit DORMANCY. Exogenous dormancy
is that due to the effects of environmental conditions; germination occurs only under conditions favourable for vegetative
growth. Endogenous (= constitutive) dormancy is due to internal factors; these may include (a) the presence of a permeability barrier to nutrients, (b) the existence of a (reversible)
metabolic block, and/or (c) the presence of an endogenous
chemical inhibitor of germination. The self-inhibitor in e.g.
uredospores of Puccinia graminis is methyl-cis-ferulate (which
inhibits removal of the germination plug in the spore wall), while
in the uredospores of some other rusts the inhibitor is methylcis-3,4-dimethoxycinnamate (which blocks initiation of the germ
tube). In general, self-inhibitors may account for the low rate of
germination of spores in masses; the leaching of inhibitor may
account for the enhancement in germination when such spores
are washed with water.
Dormancy can be broken by activation e.g. by certain
chemical agents (activators) that include detergents and organic
solvents; by heating the spores to ca. 5060 C for 1020 min
(e.g. Neurospora spp); or by subjecting the spores to cold (e.g.
teliospores of Puccinia graminis). Some spores can be induced
to germinate by damaging the spore wall.
[Physiology and biochemistry of fungal sporulation: ARPpath.
(1982) 20 281301.]
Protozoal spores. See e.g. ASCETOSPORA; MICROSPORA; MYXOZOA.
spore ball See USTILAGINALES.
spore coat
sporoactinomycetes A category within the order ACTINOMYCETALES which includes spore-forming organisms that are characterized by a morphology more complex than that of the
NOCARDIOFORM ACTINOMYCETES.
Sporobolomyces A genus of fungi (see SPOROBOLOMYCETACEAE)
which form spheroidal, ovoid or elongate budding yeast cells;
some species can form pseudomycelium and true mycelium.
The cell walls lack xylose, and growth on malt agar is pink,
red or orange due to the presence of carotenoid pigments
(cf. BULLERA). Ballistospores are formed on hyphal and yeast
cells; they are typically bilaterally symmetrical (e.g. reniform or
sickle-shaped) and develop obliquely at the tips of branched
or unbranched sterigmata. Metabolism is strictly respiratory.
NO3 is assimilated by S. holsaticus, S. puniceus (formerly
Candida punicea), S. roseus and S. salmonicolor, but not by
S. albo-rubescens, S. gracilis or S. shibatanus. Species may be
anamorphs of SPORIDIOBOLUS spp; they have been isolated e.g.
from plant material, from beer (S. roseus), etc. [Book ref. 100,
pp. 911920.]
Sporobolomycetaceae A family of anamorphic fungi (see BLASTOMYCETES) which are characterized by the formation of BALLISTOSPORES. The organisms, which have basidiomycetous affinities, form budding yeast cells; some can form pseudomycelium
and/or true mycelium. The family includes BULLERA and
SPOROBOLOMYCES. (See also MIRROR YEASTS.)
sporocarp Syn. FRUITING BODY.
Sporochnus See PHAEOPHYTA.
sporocladium See KICKXELLALES.
sporocyst (1) In most coccidia: a sac, formed within an oocyst,
containing one or more (often 2, 4 or 8) sporozoites; there
may be one or more sporocysts per oocyst. Sporocysts may be
ovoid, spherical or elongated, and those of some species have a
STIEDA BODY. (See also EIMERIORINA and SPORULATION.) (2) See
MONOCYSTIS.
Sporocytophaga A genus of GLIDING BACTERIA of the CYTOPHAGALES. The cells are pigmented rods, up to ca. 8 m long,
from which resting cells (microcysts) develop; the microcyst
is a spherical, desiccation-resistant structure which has a thick
capsule. The organisms are chemoorganotrophic; growth occurs
aerobically on cellulose (see CELLULASES), cellobiose, or glucose
(mannose is used by some strains). Growth is inhibited by high
concentrations of organic nitrogen or of sugars.
sporodochium A pad- or cushion-like fungal STROMA which
bears a surface layer of conidiophores. Sporodochia are formed
e.g. by species of Fusarium and Nectria.
sporogony (1) The division of a zygote (= sporont ) into a
number of haploid cells (sporozoites). (2) The (mitotic) division
of a cell (sporont) into a number of spores or sporozoites. (3) A
process which involves the formation and fusion of gametes and
the division of the zygote to form spores or sporozoites.
Sporolactobacillus A genus of Gram-positive, chemoorganotrophic, microaerophilic, catalase-negative, ENDOSPORE-forming
bacteria which occur e.g. in soil. Cells: flagellated rods, ca.
1 35 m. Lactic acid is formed, anaerogenically, from e.g.
glucose and other sugars and from sugar alcohols. Type species:
S. inulinus.
Sporomusa A genus of Gram-negative, anaerobic, ENDOSPOREforming bacteria isolated e.g. from river-mud, soil, waste water
etc. Cells: mainly banana-shaped, motile (with up to 15 lateral
flagella). The organisms can use e.g. N-methyl compounds
(e.g. betaine, sarcosine), primary alcohols, hydroxy fatty acids,
and 2,3-butanediol as substrates, acetate being the characteristic
product of metabolism; H2 and CO2 are converted to acetate.
nodules are formed often in a line following a lymphatic vessel; the nodules eventually ulcerate, and lymphangitis may occur.
Occasionally, internal organs may be infected. Potassium iodide
has been used for treatment.
Sporotrichum A genus of fungi of the HYPHOMYCETES. S. pulverulentum is the anamorph of the WHITE ROT basidiomycete
Phanerochaete chrysosporium.
Sporozoa A subphylum of parasitic protozoa comprising the
classes Telosporea, Toxoplasmea and Haplosporea [JP (1964)
11 720]; organisms in this taxon (excluding those of the
Haplosporea) have since been classified, with the piroplasms,
in the APICOMPLEXA.
Sporozoasida A class of protozoa of the phylum APICOMPLEXA
(q.v. for ref.) in which the APICAL COMPLEX is generally well
developed, and the conoid, when present, forms a complete
truncate cone; typically, cyst formation and both sexual and
asexual reproduction occur. Motility involves e.g. cell flexion;
the microgametes of some species are flagellated. Some species
are parasitic in vertebrates, some in invertebrates. Subclasses:
COCCIDIASINA, GREGARINASINA and PIROPLASMASINA.
Sporozoea A class of protozoa [JP (1980) 27 3758] equivalent
to the SPOROZOASIDA.
sporozoite See SPOROGONY.
sporulation (1) The process of development of a SPORE (see e.g.
ENDOSPORE sense 1(a)).
(2) In coccidia: the formation, within the oocyst, of (haploid)
sporozoites from the zygote (see EIMERIORINA); in most species
the sporozoites are formed in SPOROCYSTS. In many species
(e.g. most Eimeria spp) sporulation occurs outside the host,
i.e. only unsporulated oocysts are found in fresh faeces; for
identification purposes the oocysts in faeces can be concentrated
(e.g. by FLOTATION) and sporulated in a 23% solution of
potassium dichromate for 27 days at e.g. 2030 C. (cf.
ENDOSPORULATION.)
spoT gene
In Escherichia coli : a gene encoding an enzyme
which can synthesize and degrade ppGpp.
spotted fevers A group of human rickettsioses which includes
e.g. ROCKY MOUNTAIN SPOTTED FEVER, BOUTONNEUSE, QUEENSLAND
TICK TYPHUS and RICKETTSIALPOX. In spotted fevers the rash
develops first on the extremities, later on the trunk. (In TYPHUS
FEVERS and SCRUB TYPHUS the rash appears first on the trunk,
later on the extremities.)
spotted sickness Syn. PINTA.
spp Plural form of sp (q.v.).
SPR See BIACORE.
spraing A POTATO DISEASE caused either by the tobacco rattle
virus (see TOBRAVIRUSES) or the potato mop top virus (see
TOBAMOVIRUSES). TRV causes brown, crescent-shaped corky
regions to develop in the tubers, and small yellow rings to form
on the leaves. PMTV may cause e.g. yellowish or brown Vshaped lesions on leaves, and crescent-shaped lesions within
tubers.
spread plate (1) A method of INOCULATION: a liquid INOCULUM
(e.g. 0.050.1 ml) is spread over the surface of a dried PLATE
with a sterile SPREADER or SWAB; the inoculated plate is then
dried before incubation. The spread plate procedure is used e.g.
as a COUNTING METHOD. (2) A plate inoculated as in (1).
spreader A simple L-shaped tool used in preparing a SPREAD
PLATE; it can easily be made by fusing the tip of a Pasteur pipette
and bending the fine-bore tube to a convenient angle.
spreading factor Syn. HYALURONATE LYASE.
spring viraemia of carp (German INFECTIOUS DROPSY) A FISH
DISEASE important among cultured carp (Cyprinus carpio) in
731
springer
has tyrosine-specific protein kinase activity. The c-src product
also has tyrosine kinase activity, but c-src is expressed at very
low levels in most normal cells; cells transformed by RSV usually contain relatively high levels of pp60vsrc . The c-src and
v-src products are similar but not identical, differing in their Cterminal amino acid sequences; this difference in structure may
be at least partly responsible for the transforming capacity of
pp60vsrc [Book ref. 113, pp. 1925].
SrfI See RESTRICTION ENDONUCLEASE (table).
SRID Single radial immunodiffusion: see SINGLE DIFFUSION.
sRNA Soluble RNA, an early term for tRNA.
SRO Sex-ratio organism: any of several strains of Spiroplasma
(serogroup II) which can infect Drosophila spp, inducing a trait
in which infected female flies produce only female progeny.
SROs can be transmitted transovarially; they have not been
cultivated in vitro.
SRP SIGNAL RECOGNITION PARTICLE.
srrAB genes See AGR LOCUS.
SRSVs SMALL ROUND STRUCTURED VIRUSES.
s.s. SENSU STRICTO (q.v.).
ss (of DNA or RNA) Single-stranded.
SS agar (salmonellashigella agar) An agar medium containing
e.g. beef extract, lactose, thiosulphate, ferric citrate, bile salts,
neutral red and brilliant green [recipe: Book ref. 2, p. 137].
SS agar is used as a differential and selective medium for
salmonellae and shigellae. Colonies are pink for lactose +ve
strains, colourless for lactose ve strains; for H2 S-producing
strains, each colony has a black centre.
SSA See SUPERANTIGEN.
SSB protein SINGLE-STRAND BINDING PROTEIN.
SSC See STANDARD SALINE CITRATE.
ss(c)DNA Single-stranded circular DNA.
SSCP (single strand conformation polymorphism) SSCP analysis is a method (used e.g. for TYPING) in which related samples of
single-stranded DNA (e.g. homologous sequences from related
strains) are compared by comparing their electrophoretic speeds
in polyacrylamide gel; strands in which even one base differs may be distinguishable if this change in sequence affects
intra-strand base-pairing (conformation) in such a way that electrophoretic speed is altered. (A non-denaturing gel is used for
SSCP analysis in order to promote/preserve intra-strand basepairing.) Typically, strands of 100300 bp in length are examined by SSCP analysis.
Samples of single-stranded DNA can be produced by PCR;
such a protocol (PCR-SSCP) has been used e.g. for typing
Neisseria meningitidis [JCM (1997) 35 18091812].
PCR-SSCP has also been used e.g. for detecting point
mutations that confer resistance to the antibiotic rifampicin in
Mycobacterium tuberculosis. In this procedure, PCR amplifies a
specific mutation-prone region in the rpoB gene (which encodes
the b subunit of RNA polymerase the target for rifampicin);
amplicons from a given test strain are then compared, by
SSCP analysis, with the corresponding sequences from wildtype (i.e. rifampicin-sensitive) and mutant strains. Resistance to
other antibiotics can be assessed similarly by analysing relevant
sequences of the genome; in one study, SSCP analysis was used
for detecting resistance to rifampicin and isoniazid by examining
four chromosomal loci [JCM (1997) 35 719723].
One problem with SSCP analysis is that some silent mutations
produce conformations that simulate those of resistant strains,
giving rise to false-positive results [JCM (1997) 35 492494].
(See also DGGE.)
ssDNA phage (single-stranded DNA phage) Any BACTERIOPHAGE
which contains ss cccDNA: see INOVIRIDAE and MICROVIRIDAE.
staining
ssDNA phages are widely studied as models for bacterial DNA
Replication of the phage genome involves three
stages. Stage I: synthesis of a complementary (c or minus)
strand on the viral (v or plus) ss cccDNA to form a ds cccDNA
replicative form (RF). Stage I requires only host proteins and
involves the synthesis of RNA primer(s) on SINGLE-STRAND BINDING PROTEIN-coated v DNA by one of three mechanisms (see
INOVIRUS, BACTERIOPHAGE G4, BACTERIOPHAGE fX174); primers
are elongated with DNA by host DNA POLYMERASE III holoenzyme, and the RNA is then excised and replaced with DNA by
host DNA polymerase I. The ends of the c strand are then joined
by DNA ligase. Stage II: semiconservative replication of RF to
yield progeny RF. Usually the v strand is nicked at a specific site
by a phage-coded enzyme (cf. BACTERIOPHAGE G4); elongation of
the 3 -end thus formed is carried out by host DNA polymerase
III holoenzyme (using c strand as template) in a ROLLING CIRCLE
MECHANISM, the RF strands being unwound by host Rep protein
(see HELICASES). The displaced v strand serves as template for c
strand synthesis. Stage III: asymmetric synthesis in which only
v ss cccDNA is produced from RF. This stage requires phagecoded proteins (see INOVIRUS and BACTERIOPHAGE fX174). [DNA
replication in ssDNA phages: BBA (1985) 825 111139.]
SSF Simultaneous saccharification and fermentation: a batchtype process in which dextrins are enzymically hydrolysed to
glucose (saccharification), the glucose being immediately taken
up and fermented by organisms in the dextrin solution.
SSM Simple matching coefficient. In the mutual comparison of
two OTUs by NUMERICAL TAXONOMY: the number of characteristics which match i.e. which are the same (both positive or
both negative) in the given pair of OTUs, expressed as a percentage of the total number of characteristics (criteria) used in
the comparison. SSM can be used only when the characteristics
can be expressed in simple, discontinuous form, e.g. + or , 0
or 1 (cf. entry SG ).
ssp Subspecies.
SsrASsrB See TWO-COMPONENT REGULATORY SYSTEM.
SSSS Staphylococcal SCALDED SKIN SYNDROME.
SST See STANDARD TESTS FOR SYPHILIS.
ST See ETEC.
St Anthonys fire (1) Syn. ERGOTISM. (2) Syn. ERYSIPELAS.
St Louis encephalitis (SLE) An acute, viral ENCEPHALITIS caused
by a flavivirus (see FLAVIVIRIDAE); it occurs in epidemics in urban
regions of central and southern USA. The virus is prevalent in
wild birds and is transmitted by Culex spp (mosquitoes) which
feed on birds and man. The disease may be benign with few
sequelae, but can be fatal, particularly in the elderly.
St Vituss dance See RHEUMATIC FEVER.
ST-I Syn. STa (see ETEC).
ST-II Syn. STb (see ETEC).
STa Syn. ST-I (see ETEC).
sta locus See PARTITION.
STAA medium A selective medium used e.g. for isolating
Brochothrix thermosphacta from meat and meat products; it
consists of a basal growth medium containing streptomycin,
thallous acetate and Actidione (cycloheximide).
stab culture See CULTURE.
stabilate A population of viable microorganisms preserved by
FREEZE-DRYING or by FREEZING so that their characteristics remain
unchanged. (Populations preserved by repeated subculture are
subject to genetic change by selection of mutants.)
stabilized erythrocyte See HAEMAGGLUTINATION.
stable RNA In prokaryotes: a term sometimes used to refer
to rRNA and tRNA as opposed to the (typically) short-lived
mRNA.
REPLICATION.
733
staling
with phage typing, prevent the clumping factor reaction (in the
COAGULASE TEST), and affect the morphology of the colony.)
Most species appear to contain only a- and b-type CYTOCHROMES
(c-type cytochromes occur in S. sciuri ) [Book ref. 44, p 399].
Staphylococci occur as commensals/parasites and pathogens
in man and other animals. Diseases caused by species of
Staphylococcus in man and animals include e.g. ARTHRITIS,
BLACK POX, BOIL, BRONCHITIS, BUMBLEFOOT, CARBUNCLE, CYSTITIS,
ENDOCARDITIS, FOOD POISONING, IMPETIGO, JOINT-ILL, KERATOCONJUNCTIVITIS, MENINGITIS, OSTEOMYELITIS, PNEUMONIA, SCALDED
SKIN SYNDROME and TOXIC SHOCK SYNDROME. (See also EAR
MICROFLORA, GENITOURINARY TRACT FLORA, RESPIRATORY TRACT
MICROFLORA, SKIN MICROFLORA, VAGINA MICROFLORA.)
GC%: ca. 3039. Type species: S. aureus.
Classification of the staphylococci. Staphylococci are divided
into COAGULASE-positive and coagulase-negative strains. Strains
of S. aureus and S. intermedius are coagulase-positive, as are
some strains of the animal pathogen S. hyicus subsp hyicus;
most species of Staphylococcus are coagulase-negative. In terms
of pathogenic potential, S. aureus is considered to be the most
important species; however, other species, including a number
of coagulase-negative staphylococci (CNS), are also associated
with disease, often as opportunist pathogens.
Species include:
S. albus. See S. epidermidis.
S. aureus. A major pathogen of man and other animals. The
cells, ca. 1 m in diam., are often pigmented (see STAPHYLOXANTHIN), particularly in freshly isolated strains. The cell wall
usually contains ribitol teichoic acids, and most strains form
PROTEIN A; the PEPTIDOGLYCAN contains little or no L-serine. The
cell wall lipoteichoic acid is a virulence factor: it acts as an
adhesin which binds to fibronectin (a glycoprotein component
of e.g. epithelial cells). Protein adhesins of S. aureus bind to
mammalian targets such as collagen and fibronectin [TIM (1998)
6 484488]. (See also SORTASE.)
The expression of virulence factors by S. aureus is controlled
by various mechanisms which involve e.g. the AGR LOCUS.
The expression of certain virulence factors, including exotoxin,
appears to involve a TWO-COMPONENT REGULATORY SYSTEM that
responds to levels of environmental oxygen [JB (2001) 183
11131123].
In general, the expression of virulence factors in S. aureus
depends on the growth phase and/or on conditions of growth.
Regulation of exotoxins and wall-associated proteins (e.g. PROTEIN A) is complex [FEMS Reviews (2004) 28 183200].
The organism forms a thermostable DEOXYRIBONUCLEASE, and
produces both free coagulase and clumping factor (see COAGULASE and COAGULASE TEST). [Evaluation of the STAPHYLOSLIDE
and other agglutination tests: JCM (1985) 21 726729.] All
strains coagulate e.g. human and rabbit plasma.
Glucose is usually fermented to DL-lactic acid, and lactose
metabolism involves the tagatose 6-phosphate pathway (see
Appendix III(a)). Mannitol is utilized aerobically and anaerobically, and maltose is utilized aerobically. VP +ve. (See also
HYALURONATE LYASE and PHOSPHATASE.)
S. aureus is characteristically sensitive to NOVOBIOCIN (MIC
<1.6 g/ml). Most strains are resistant to benzylpenicillin
(owing to the action of staphylococcal b-LACTAMASES), and
some strains are resistant to methicillin (see MRSA). MRSA has
been detected by multiplex PCR, target sequences being in mecA
(encoding PBP 2a) and the coa gene (encoding coagulase, and
used as a marker for S. aureus) [JMM (1997) 46 773778].
Staphylococcus
Antibiotics that have been used therapeutically against
S. aureus include various b-lactams (e.g. flucloxacillin), clindamycin, erythromycin and vancomycin.
S. aureus is susceptible to effective concentrations of
phenolic disinfectants, HYPOCHLORITES, CHLORHEXIDINE and
povidoneiodine (see IODINE). The organism can withstand
60 C/30 min. The D VALUE of S. aureus at 70 C is often less
than 1 minute (although much longer in some strains).
S. aureus has been divided into four biotypes: AD (biotypes
E and F are now classified as S. intermedius). The biotypes
usually correlate with source: man (A), poultry and pigs (B),
bovines and sheep (C), and hares (D). The biotypes of S. aureus
are distinguishable e.g. by FIBRINOLYSIN production (A strains
only); coagulation of bovine plasma (C strains only); formation
of a-haemolysin (see HAEMOLYSIN, sense 2e) (A strains, some
B and C strains); formation of b-haemolysin (C and D strains,
most B strains, few A strains); mannitol fermentation within 5
days (A and B strains, some C strains).
PHAGE TYPING of S. aureus is carried out with five groups of
phages. A strain of S. aureus which can be lysed by phage(s)
of lytic group I is referred to as S. aureus phage type I; a strain
lysed by phage(s) of group II is referred to as S. aureus phage
type II etc. A given strain may be lysed by the phages of more
than one group; for example, many of the (phage-typable) strains
of MRSA are lysed by phages of groups I and III (while other
strains of MRSA may be lysed by group III phages only). The
phages used for typing S. aureus have been standardized: they
belong to the international set; for example, group I phages
include those designated 29, 52, 52A, 79 and 80. The phages of
group IV are used for typing isolates of S. aureus derived from
animals. (Some strains of Staphylococcus are not typable by this
system; such strains presumably lack the receptors for relevant
phages.)
S. aureus can also be typed by MLST [database: JCM (2000)
38 10081015]. A further method is PCR-RFLP with a speciesspecific target e.g. a sequence in the gene aroA (which encodes
the enzyme 5-enolpyruvylshikimate-3 phosphate, used in the
synthesis of aromatic amino acids and folate) [JCM (1999) 37
570574]. Other typing methods include PFGE. [A comparison
of PFGE with five other molecular methods for typing S. aureus
(MRSA): JMM (1998) 47 341351.]
S. capitis. Coagulase-negative. The cell wall contains glycerol
teichoic acids. Sensitive to novobiocin (MIC <1.6 g/ml). Acid
is not formed, aerobically, from e.g. maltose, trehalose or
melezitose. Occurs e.g. on the normal human scalp, but has been
associated with several cases of infective endocarditis and with
urinary tract infections.
S. caprae. [Original species proposal: IJSB (1983) 33
480486.] Isolated from both animal and human specimens.
Evidence for pathogenicity in man [see e.g. RMM (1995) 6
94100 (97)].
S. carnosus. [Original species proposal: IJSB (1982) 32
153156.]
S. caseolyticus. [Original species proposal: IJSB (1982) 32
1520.]
S. cohnii. Coagulase-negative. The cell wall contains glycerol
teichoic acids. Resistant to novobiocin (MIC 1.6 g/ml). Acid
is not formed, aerobically, from sucrose or melezitose. Occurs
on human skin.
S. epidermidis (formerly S. albus). Coagulase-negative. The
cell wall contains glycerol teichoic acids. Novobiocin-sensitive
(MIC <1.6 m/ml). Acid is not formed, aerobically, from
L-arabinose, D-mannitol, trehalose or D-xylose but is produced from sucrose. Anaerobic growth occurs in thioglycollate
staphylokinase
stationary phase (of growth) See BATCH CULTURE.
statismospore (mycol.) A spore which is not forcibly discharged.
(cf. BALLISTOSPORE.) In basidiomycetes, a BASIDIOSPORE which is
a statismospore is either formed in a symmetrical orientation on
its sterigma, or it is formed directly from the basidium, i.e., with
no sterigma. (cf. GASTEROID BASIDIOSPORE.)
staphylokinase A protein, produced by many strains of coagulase-positive staphylococci, which activates profibrinolysin (from
various species) to fibrinolysin, thus causing indirect FIBRINOLYSIS. Its mechanism of action appears to be similar to that of STREPTOKINASE. [Assay, properties etc: Book ref. 44, pp. 790796.]
staphylomycins See STREPTOGRAMINS.
Staphyloslide A test used to detect clumping factor (see COAGULASE) in strains of Staphylococcus aureus; essentially, a given
strain is examined (on a slide) for its ability to clump fibrinogencoated sheep erythrocytes.
Staphylothermus A genus of heterotrophic, coccoid archaeans.
The type species, S. marinus, grows optimally at ca. 92 C under
anaerobic conditions; it was isolated from a HYDROTHERMAL
VENT. [Book ref. 196, pp. 6971.]
staphylothrombin See COAGULASE.
staphyloxanthin The main CAROTENOID pigment in Staphylococcus aureus. [Structure and synthesis: JB (1981) 147 900919.]
star activity (of a restriction endonuclease) A change, or reduction, in the specificity of certain RESTRICTION ENDONUCLEASES
(e.g. BamHI, EcoRI, SalI) which occurs under non-optimal conditions.
starch A composite D-glucan consisting of amylose (ca.
2025%, depending on source) and amylopectin. Amylose is
a water-soluble linear (1 4)-a-D-glucan which forms blueblack complexes with iodine. Amylopectin is a highly branched
(1 4)-a-D-glucan with (1 6)-a-D-glucosidic branch points;
it is water-insoluble and forms violet or red-brown complexes
with iodine (cf. GLYCOGEN). Starch is abundant as the main
storage carbohydrate in higher plants and in certain algae,
e.g., members of the Chlorophyta (chlorophycean starch); an
amylose-like glucan occurs in the cell walls of certain fungi,
and yeasts of the genus Cryptococcus characteristically form
an extracellular CAPSULE of an amylose-like polysaccharide.
(See also CYANOPHYCEAN STARCH; FLORIDEAN STARCH; LICHENIN.)
Starch may be stained e.g. with iodine or (non-specifically) by
the PAS REACTION.
Starch is attacked by a wide range of microorganisms (see e.g.
AMYLASES and DEBRANCHING ENZYMES). That from higher plants
is an important raw material for a number of biotechnological
processes see e.g. INDUSTRIAL ALCOHOL and SINGLE-CELL PROTEIN.
STARFISH A water-soluble multivalent carbohydrate ligand
(a starfish-shaped molecule) which can bind to, and neutralize, the shiga-like toxins (SLT-I and SLT-II) of Escherichia
coli O157:H7 with subnanomolar activity; the structure of
STARFISH is related to that of the (glycolipid) toxin-binding
sites (Gb3 ) on mammalian vascular endothelium. (See also SYNSORB Pk .) [STARFISH: Nature (2000) 403 669672.]
starlingpox virus See AVIPOXVIRUS.
Starria A genus of filamentous CYANOBACTERIA in which the
trichomes are triradiate in cross-section; S. zimbabweensis has
been recorded in only one geographical location. [J. Phycol.
(1977) 13 288296.]
start (in cell cycle) See CELL CYCLE.
start point (start site) See TRANSCRIPTION.
starter (starter culture) An INOCULUM, usually consisting of a
pure or mixed culture of microorganisms, used to initiate a commercial FERMENTATION (sense 2) (see e.g. LACTIC ACID STARTERS).
Starter cultures are often grown under aseptic conditions in a
laboratory (but cf. e.g. KEFIR and sourdough BREAD-MAKING).
State 3, State 3u, State 4 (bioenergetics) See RESPIRATORY CONTROL.
stathmokinesis Inhibition of cell division (e.g. by COLCHICINE).
736
sterile
(unlike any other known ciliate) the possession of only one type
of nucleus.
Stephanopyxis See DIATOMS.
sterco- Indicates a connection with faeces, e.g., stercorous:
resembling faeces.
Stercoraria One of two groups of subgenera of mammalian
trypanosomes; stercorarian trypanosomes infective for the vertebrate host develop in the POSTERIOR STATION. The group
comprises HERPETOSOMA, MEGATRYPANUM and SCHIZOTRYPANUM.
(cf. SALIVARIA.)
Stereaceae See APHYLLOPHORALES.
Stereocaulon A genus of LICHENS (order LECANORALES); photobiont: a green alga. Erect pseudopodetia (see PSEUDOPODETIUM) typically richly branched and fruticose, covered with
scale-like, finger-like or coralloid outgrowths (phyllocladia)
arise from a granular, usually rapidly evanescent primary thallus. Dark-brown apothecia may occur terminally or laterally on
the pseudopodetia, and dark-coloured cephalodia are commonly
present. Species occur on soil and rocks, some being associated
with habitats rich in heavy metals.
stereocilium Syn. CLAVATE CILIUM.
Stereomyxa See ACARPOMYXEA.
Stereum A genus of lignicolous fungi of the APHYLLOPHORALES
(family Stereaceae) which form typically resupinate or effusedreflexed, leathery or woody fruiting bodies in which the context
lacks clamp connections and is usually dimitic. (See also PAPER
SPOILAGE, PARTRIDGE WOOD, WOODWASP FUNGI and XYLANASES.)
Steriflamme process A form of heat treatment used for canned
foods (see CANNING). Cans are initially heated to a given
temperature by steam at atmospheric pressure. The rapidly
spinning cans are then exposed directly to gas flames so that
their contents are quickly heated to ca. 120130 C. The cans
are held at the processing temperature for the required time and
are then cooled by water sprays.
sterigma (pl. sterigmata) (mycol.) (1) In certain fungi: a small
or substantial protrusion from which a spore or daughter cell is
produced see e.g. BASIDIUM and STERIGMATOMYCES. (See also
SPICULUM.)
(2) See ASPERGILLUS.
sterigmatocystin A carcinogenic, hepatotoxic MYCOTOXIN which
contains a bifuran moiety fused at the 4,5 positions to a
substituted xanthone (cf. AFLATOXINS); it is produced e.g. by
Aspergillus nidulans and A. versicolor.
Sterigmatomyces A genus of fungi (class HYPHOMYCETES) which
form spherical to ovoid yeast cells and which may form a
true mycelium. A vegetative cell produces one or more fine
projections (sterigmata), at the end of each of which a daughter
cell forms by budding. When mature, the daughter cell may
in turn produce sterigmata, often resulting in the formation
of short, branching chains of cells; cells may separate by the
formation of a septum in the middle or at the distal end of the
sterigma, according to species. Metabolism is strictly respiratory.
Six species are recognized; type species: S. halophilus. [Book
ref. 100, pp. 921929; cell cycle in S. halophilus: JGM (1983)
129 21292162.]
sterilant Any chemical agent which, under carefully controlled
conditions, can sterilize objects, materials etc (see STERILIZATION;
cf. DISINFECTANT); examples include e.g. ETHYLENE OXIDE, GLUTARALDEHYDE, b-PROPIOLACTONE (cf. FORMALDEHYDE). If conditions are not carefully controlled, a sterilant may fail to sterilize
[JAB (1983) 54 9199]. (cf. BIOCIDE.)
sterile (1) Refers to the condition of an object, or an environment, which is free of all living cells, all viable spores (and
sterile cabinet
heating with a bactericide. (See also e.g.
other resistant and disseminative forms), and all viruses and subviral agents capable of replication. (An effective STERILIZATION
process must therefore irreversibly inactivate all organisms.) For
most practical purposes the main criterion of sterility is satisfied
by the failure to detect viable cells, spores, viruses etc on or in a
given object, material or environment; it should be appreciated
that a viable organism can be detected only if it is provided with
conditions suitable for its growth or replication or other form of
expression.
(2) Refers to any structure or tissue which does not or cannot
have a reproductive function.
sterile cabinet Syn. SAFETY CABINET.
sterile immunity Syn. STERILIZING IMMUNITY.
sterile pyuria See PYURIA.
sterile technique Syn. ASEPTIC TECHNIQUE.
sterility The state or condition of being STERILE. (cf. COMMERCIAL
STERILITY.)
sterilization (1) Any process by which objects, materials, or
environments may be rendered STERILE (sense 1). (Since sterility
is an absolute condition, the expression partial sterilization is
meaningless cf. DISINFECTION.) When contaminating organisms
are known to consist entirely of vegetative or other vulnerable
forms, sterility can usually be achieved by mild heat or chemical
treatments; however, sterilization commonly refers to those
processes which guarantee sterility regardless of the nature of
the contaminating microflora.
(a) Methods of sterilization.
(i) Physical methods. Heat is the most reliable (and generally
the preferred) sterilizing agent; it can reach organisms that may
be protected from the action of chemical sterilizing agents or
from radiation. The lethal action of heat is due largely to the
denaturation of microbial proteins and nucleic acids and to the
lability of membranes; at sterilizing temperatures nucleic acids
may be deaminated, depurinated or otherwise degraded.
Dry heat. Sterilization of clean glassware etc may be carried
out in a HOT-AIR OVEN (q.v.); under such conditions proteins
are denatured, cytoplasm desiccated, and various cell and virus
components are oxidized. Infrared radiation (l within the
range 7.5 105 to 4 102 cm) has been used e.g. for the
sterilization of small items of medical glassware. Incineration
(combustion) is used e.g. for the disposal of used surgical
dressings, and is the basis of FLAMING.
Moist heat (steam) is more rapidly lethal than dry heat at
the same temperature. The relative ease with which moist heat
denatures proteins may be due to facilitated rupture of the
protein-stabilizing hydrogen bonds; these bonds are broken more
easily when water molecules are available for hydrogen bonding.
Moist heat also effects an efficient transfer of heat since steam
which condenses on a cooler object (during the heating-up
period) delivers up a large amount of latent heat. Moist heat
sterilization is generally carried out in an AUTOCLAVE (q.v.).
Radiation. See IONIZING RADIATION; MICROWAVE RADIATION;
ULTRAVIOLET RADIATION.
Filtration. See FILTRATION.
Ultrasonication. ULTRASONICATION may achieve sterility in
some cases, but it is not a reliable method of sterilization.
(ii) Chemical methods. Among the few reliable STERILANTS are
ETHYLENE OXIDE, GLUTARALDEHYDE and b-PROPIOLACTONE; such
agents must be used in effective concentrations under carefully
controlled conditions.
(iii) Combined physical and chemical methods. In the pharmaceutical industry, the vapour of e.g. chlorocresol (see PHENOLS) is used at 98100 C in a procedure that has been called
LOW-TEMPERATURE
STEAMFORMALDEHYDE STERILIZATION.)
(b) Kinetics of sterilization (some basic ideas). In a singlespecies microbial population, the death rate produced by many
types of lethal agent (including heat, radiation, various chemical
disinfectants and sterilants) follows approximately first-order
kinetics. However, close approximations to first-order kinetics
are obtained only when sterilizing temperatures are relatively
high, or when disinfectants or sterilants are used in relatively
high concentrations. Under these conditions, the decrease in
numbers of microbial contaminants may be summarized by the
equation:
loge N0 loge N = kt
where N0 is the initial number of viable organisms, N is the
number of survivors at time t, and k is the death rate constant.
For a given organism, different values of k can be obtained for
different sterilizing temperatures or different concentrations of
a disinfectant or sterilant. In a mixed microbial population the
cells will have different degrees of resistance to heat, chemicals
etc, and a sterilization process will not follow first-order kinetics;
in such cases the curve obtained by plotting loge N versus t (to
find k) will be a composite curve.
(See also APPERTIZATION; DISINFECTION; D VALUE; F0 VALUE;
MPED; THERMAL DEATH POINT; THERMAL DEATH TIME; Z VALUE.)
(2) (med., vet.) Complete elimination of a parasite or pathogen
from a host either by the immune response (see STERILIZING
IMMUNITY) or by chemotherapy.
sterilizer (1) Any apparatus used for STERILIZATION, e.g., an
AUTOCLAVE or a HOT-AIR OVEN. (2) A STEAMER. (3) Any of
certain types of apparatus used in the CANNING industry for
APPERTIZATION.
sterilizing immunity (sterile immunity) An immune response
which results in the total elimination of a parasite or pathogen
from the body. (cf. PREMUNITION.)
Sterne strain A toxin-producing strain of Bacillus anthracis
which lacks the poly-D-glutamic acid capsule; it is used as a
live vaccine against ANTHRAX. The lack of a capsule allows the
elimination of the organism by phagocytosis.
steroid bioconversions Certain steroid hormones and related
compounds are produced commercially by a process in which
most of the steps are effected chemically, but some rely on
the selective action of certain microorganisms; the microbial
reactions have the advantages of being site-specific and stereospecific Examples. Production of corticosteroid hormones (e.g.
cortisol) involves the chemical conversion of stigmasterol (from
various plants) or diosgenin (e.g. from yams) to progesterone; the
11a-hydroxylation step is achieved e.g. by Rhizopus nigricans
or Aspergillus spp. (The remainder of the synthesis is achieved
chemically.) In the synthesis of testosterone, the reduction of
4-androstene-3,17-dione to the 17b-hydroxy derivative can be
achieved e.g. by strains of Saccharomyces cerevisiae. [Book
ref. 31, pp. 369465.] (See also CHOLESTEROL OXIDASE and BILE
ACIDS.)
Ster-zac See BISPHENOLS.
stibamine See ANTIMONY.
stibanilic acid See ANTIMONY.
stibophen See ANTIMONY.
stichobasidial Refers to a longitudinal arrangement of nuclear
spindles in a developing BASIDIUM. (cf. CHIASTOBASIDIAL.)
Stichococcus A genus of freshwater or terrestrial green algae
(division CHLOROPHYTA) which are apparently closely related
to KLEBSORMIDIUM. When undisturbed, the organisms grow as
738
stomatogenesis
Stigonematales See CYANOBACTERIA.
stilbaceous Having synnemata.
Stilbellales See HYPHOMYCETES.
Stilton cheese See CHEESE-MAKING.
stimulatory hypersensitivity Syn. TYPE V REACTION.
stinkhorns See PHALLALES.
stinking smut Syn. bunt: see COMMON BUNT and KARNAL BUNT.
stipe A stalk or stem. In e.g. an agaric-type fungal fruiting body
the stipe is composed of hyphae which are characteristically
orientated parallel to the axis of the stipe (cf. receptacle in
PHALLALES). In PENICILLIUM spp stipe refers to the (single)
hypha which supports the penicillus.
stipitate Having a STIPE.
stirred tank reactor (STR) A FERMENTER in which the culture
is agitated by a mechanical device (e.g. a turbine) but in which
there is no circulatory loop (cf. LOOP FERMENTER). The traditional
STR is a squat, cylindrical vessel, but the multistage STR is a
tall (column) fermenter in which the mechanical agitators are
arranged in a vertical series on a common drive shaft. The STR
is generally more flexible than other fermenters, i.e., it is suitable
for a wider range of operating conditions.
STLV SIMIAN T-CELL LEUKAEMIA VIRUS.
stn gene See FOOD POISONING (Salmonella).
stock Any uncharacterized population of trypanosomes derived
from a natural host animal; a given stock may contain different
strains of trypanosomes.
Stoffel fragment See DNA POLYMERASE.
stolon (mycol.) See e.g. RHIZOPUS.
stomach (human) See GASTROINTESTINAL TRACT FLORA.
stomate Having a mouth, stoma(ta), or CYTOSTOME.
stomatitis Inflammation of the tissues of the mouth. The causes
of stomatitis include e.g. irritation of the tissues by ill-fitting
dentures, vitamin deficiency, and infection by any of a range
of microorganisms: see e.g. CANDIDIASIS, GINGIVITIS, HAND FOOT
AND MOUTH DISEASE, HERPES SIMPLEX (oral herpes), PERIODONTITIS
and VINCENTS ANGINA. (See also LUDWIGS ANGINA.)
Stomatochroon A genus of obligately endophytic algae related
to TRENTEPOHLIA. The organisms typically inhabit the stomata of
leaves, their prostrate filaments growing between the cells of the
leaf mesophyll.
Stomatococcus
A genus of facultatively anaerobic, Grampositive cocci of the family MICROCOCCACEAE. S. mucilaginosus,
the sole species, occurs in the human mouth; it has been associated with endocarditis and (in immunosuppressed individuals)
with bacteraemia. Catalase weakly +ve. Oxidase ve. Carbohydrate metabolism: fermentative. Colonies are small, dark and
mucoid. The cells are resistant to LYSOSTAPHIN. Unlike Staphylococcus, the organism is sensitive to bacitracin.
stomatogenesis The formation of the oral structures and infrastructures during the overall process of binary fission in a stomate
ciliate; morphogenetic details particularly the origin of kinetosomes of the new oral region differ among the various groups
of ciliates. There are four principal modes of stomatogenesis:
apokinetal, buccokinetal, parakinetal and telokinetal (listed in the
order which approximates an evolutionary sequence from most
advanced to most primitive). Apokinetal (de novo) stomatogenesis involves the appearance of a group of oral kinetosomes
which do not appear to have arisen either from those of the
parental oral apparatus or from those of the somatic ciliature. In
buccokinetal stomatogenesis at least some of the kinetosomes
appear to be derived from the division of kinetosomes in the
parental buccal area; in parakinetal stomatogenesis they may be
derived from kinetosomes of somatic cilia posterior to the buccal
filaments, but these readily fragment into bacilliform, uninucleate cells which each contain a single large chloroplast. Asexual
reproduction occurs by cell division and fragmentation of filaments.
stichodyad membrane See PARORAL MEMBRANE.
Sticholonche See TAXOPODIDA.
stichomonad membrane See PARORAL MEMBRANE.
stichonematic Refers to a eukaryotic FLAGELLUM which bears a
single row of fine hairs along its length.
Stickland reaction In many proteolytic species of Clostridium:
an energy-yielding reaction in which, typically, the oxidation
of one amino acid (the reductant) is coupled to the reduction
of another (the oxidant). Essentially, the reductant undergoes
oxidative deamination to an a-ketoacid (= a-oxoacid), NAD+
being reduced. The ketoacid is oxidatively decarboxylated to
a fatty acid in a reaction requiring coenzyme A and inorganic
phosphate, NAD+ being reduced and ATP synthesized. NAD+
is regenerated from NADH by the reduction or reductive
deamination of the oxidant.
Some amino acids (e.g. alanine, valine) act preferentially
as reductants, while others (e.g. glycine) act preferentially as
oxidants; according to organism, leucine and the aromatic amino
acids phenylalanine and tryptophan may act either as oxidants or
reductants. Some species (e.g. C. sporogenes) can use ornithine
by converting it to proline (an oxidant). In some cases leucine
can be used as both oxidant and reductant, and some species
can use e.g. BETAINE or sarcosine (N-methylaminoacetic acid)
as oxidant, betaine yielding acetate and trimethylamine.
sticky ends (cohesive ends) (mol. biol.) Complementary singlestranded ends of a double-stranded nucleic acid molecule generated e.g. by staggered cleavage of a circular dsDNA molecule
by certain RESTRICTION ENDONUCLEASES; base-pairing between
sticky ends of the same molecule or of two identical molecules
generates (after ligase action) cccDNA or a CONCATEMER, respectively. (See e.g. BACTERIOPHAGE l.)
Sticta A genus of foliose LICHENS (order PELTIGERALES). Photobiont: Nostoc (e.g. in S. sylvatica) or a green alga (e.g. in
S. canariensis); the mycobiont of S. canariensis can alternatively associate with a cyanobacterium to form a distinct morphotype (S. dufourii ) cf. CEPHALODIUM. Thallus: large, lobed,
corticate on both surfaces; the upper surface may bear isidia
(e.g. S. sylvatica) or soredia (e.g. S. limbata), the lower surface
is tomentose and is perforated by characteristic cyphellae (see
CYPHELLA). Species occur mainly on mossy trees and rocks.
Stieda body In some species of the APICOMPLEXA (e.g. some
Isospora spp): a structure which may form part of, or is
intimately associated with, the polar wall of the sporocyst; it
is probably involved in excystation.
stiff agar See AGAR and MEDIUM.
Stigeoclonium A genus of polymorphic, filamentous (often heterotrichous) green algae related to CHAETOPHORA. The filaments
are uniseriate, branched, and may terminate in multicellular
hyaline hairs; both prostrate and erect filaments may form rhizoids. Each cell contains a single parietal chloroplast. Reproduction is predominantly asexual, quadriflagellate zoospores and
aplanospores being produced. Sexual reproduction is isogamous.
Species occur worldwide in standing or running fresh water,
growing attached to rocks, plants, etc. (See also SEWAGE FUNGUS.)
stigma (algol.) Syn. EYESPOT (sense 1).
Stigmatella See MYXOBACTERALES.
stigmatomycosis An insect-transmitted disease of cotton (Gossypium) and other plants, caused by members of the METSCHNIKOWIACEAE (e.g. Ashbya gossypii, Nematospora gossypii ).
739
stone-brood
strawberry foot-rot A proliferative dermatitis of sheep, affecting
chiefly the lower parts of the limbs, caused by Dermatophilus
congolensis. (See also DERMATOPHILOSIS.)
strawberry latent ringspot virus See NEPOVIRUSES.
strawberry vein-banding virus See CAULIMOVIRUSES.
streak (plant pathol.) Roughly parallel lines of discoloration or
necrosis which develop on the stems or leaves of plants infected
e.g. with certain PLANT VIRUSES.
streaking INOCULATION of the surface of a solid MEDIUM in such a
way that, during INCUBATION, individual colonies form on at least
part of the surface. One method is as follows. A LOOP carrying an
INOCULUM is drawn back and forth (i.e. streaked ) on the surface
of a dried PLATE as at A (see figure). The loop is then flamed
(see FLAMING), allowed to cool, and streaked as at B. Streakings
C, D, and E are similarly made, the loop being flamed and
cooled between each streaking and after the last. In this way the
inoculum is progressively thinned out as it is distributed along
the streak lines. On incubation, each well-isolated viable cell
capable of growth on the medium gives rise to a single COLONY.
B
A
C
E
Streptococcus
not contain components which react in the Lancefield grouping
test, so that these species cannot be assigned to a Lancefield
group. (For group R see S. suis, below.)
Other components of the streptococcal cell wall (e.g. the M
PROTEIN and T PROTEIN) are also involved in streptococcal typing.
Species (and some former species) include:
S. acidominimus. Viridans streptococci, isolated e.g. from
cattle, from raw milk and from the human mouth. No Lancefield
group.
S. adjacens. See NUTRITIONALLY VARIANT STREPTOCOCCI.
S. agalactiae. Pyogenic group, isolated from man and cattle.
Lancefield group B. a-, b- and non-haemolytic strains occur,
some being pigmented. A causal agent of bovine MASTITIS (see
also CAMP TEST) and e.g. pneumonia or meningitis in human
neonates/infants. [Phage typing of S. agalactiae: Book ref. 143,
pp 122.] b-Lactam antibiotics are often used as chemoprophylaxis against infection of the neonate, while e.g. erythromycin
may be used as an alternative. However, while most strains of
S. agalactiae are currently susceptible to b-lactams, a recent
study found that >20% of 126 clinical isolates expressed resistance to macrolides. [Antibiotic susceptibility and mechanisms
of erythromycin resistance in clinical isolates of S. agalactiae (a
multicentre study): AAC (2001) 45 24002402.]
S. anginosus. See S. milleri (below).
S. avium. Lancefield group D. Typically a-haemolytic organisms which occur in the intestine in man and fowl. Referred to
ENTEROCOCCUS.
S. bovis. Lancefield group D (most strains). Strains occur e.g.
in the human gut (also found in domestic animals); infrequent
cause of endocarditis in man. (See also BLOAT; THIOPEPTIN.)
[Taxonomic study: SAAM (1984) 5 467482.]
S. canis. [Species proposal: IJSB (1986) 36 422425.] Pyogenic group, isolated from cows with mastitis and from dogs
with genital, skin or wound infections. Lancefield group G. bHaemolytic.
S. constellatus. See S. milleri (below).
S. cremoris. Lancefield group N organisms (see LACTOCOCCUS).
S. cricetus. A species isolated from hamsters (formerly
referred to as serotype a of S. mutans).
S. durans. Lancefield group D. a-, b- and non-haemolytic
strains. Referred to ENTEROCOCCUS.
S. dysgalactiae. Pyogenic group, isolated from cattle, pigs,
man. Includes strains of Lancefield groups C, G and L.
S. equi. Pyogenic group. Lancefield group C. Two subspecies:
equi and zooepidemicus. Causal agents of e.g. STRANGLES in
equines and glomerulonephritis and pharyngitis in humans. (See
also MASTITIS.)
S. faecalis. Lancefield group D. Referred to ENTEROCOCCUS.
S. faecium. Lancefield group D. Referred to ENTEROCOCCUS.
S. ferus. Oral group. Formerly referred to as strains of
S. mutans. Isolated from rats.
S. gallinarum. Lancefield group D. b-Haemolytic on horseblood agar. Occurs e.g. in the intestines of fowl. Referred to
ENTEROCOCCUS.
S. gordonii. Oral group. Organisms previously referred to as
strains of S. sanguis.
S. hyointestinalis. Pyogenic group, isolated from pigs. No
Lancefield group.
S. intermedius. See S. milleri (below).
S. lactis. Lancefield group N. Referred to LACTOCOCCUS.
Streptococcus MG. See STREPTOCOCCUS MG.
S. milleri . Streptococci associated with various types of
endogenous pyogenic infection in humans; they occur e.g. in
e.g. serum or blood. Acid (no gas) is formed from glucose and
other carbohydrates. Nitrate is not reduced. Oxidase ve. Catalase ve. GC%: ca. 2426. Type species: S. moniliformis. [Book
ref. 22, pp. 598600.]
Streptobacterium See LACTOBACILLUS.
streptobiosamine A disaccharide component of STREPTOMYCIN,
consisting of L-streptose (5-deoxy-3-formyl-L-lyxose) and 2deoxy-2-methylamino-L-glucose.
Streptococcaceae A family of Gram-positive (or Gram type
positive), asporogenous, facultatively anaerobic, chemoorganotrophic, spherical or coccoid bacteria; genera: Aerococcus,
Gemella, Leuconostoc, Pediococcus and Streptococcus [Book
ref. 21, pp. 490517].
streptococcal superantigen A See SUPERANTIGEN.
Streptococcus
A genus of Gram-positive, asporogenous,
chemoorganotrophic, facultatively anaerobic, catalase-negative
and oxidase-negative cocci or coccoid bacteria, typically ca.
1 m diam., which generally occur in pairs or chains; nonmotile. CAPSULE-formation is common in some species. Growth
usually occurs optimally in the range 3037 C. Typically
fermentative, with carbohydrates metabolized anaerogenically
and homofermentatively glucose usually yielding L-lactic acid
as the main product; however, in the presence of oxygen, some
streptococci (e.g. strains of S. mutans) can oxidize NADH by
NADH oxidase and NADH peroxidase activities [AvL (1985)
51 577578]. On blood agar some streptococci give rise to
clear HAEMOLYSIS (b-haemolysis); the VIRIDANS STREPTOCOCCI
characteristically give rise to zones of partial haemolysis with
greenish to brownish discoloration (so-called a-haemolysis).
The organisms occur as commensals/parasites and as
pathogens in man and other animals.
Streptococci are killed by PASTEURIZATION and by many
common disinfectants.
GC%: 3446. Type species: S. pyogenes.
Classification of the streptococci. Streptococcus is a large
genus (40 species) which is divided into three main groups of
species on the basis of 16S rRNA studies: the pyogenic group,
the oral group and other species.
The pyogenic group includes species associated with pyogenic infections in man and other animals e.g. S. agalactiae,
S. dysgalactiae, S. equi and S. pyogenes.
The oral group contains species (commonly isolated from the
oral cavity) which are associated with pyogenic and other infections in various sites including mouth, heart (infective endocarditis), joints, skin, muscle and central nervous system (e.g.
brain abscesses). The species in this group include S. anginosus,
S. mutans, S. oralis and S. salivarius. (See also VIRIDANS STREPTOCOCCI.) [Oral streptococci (taxonomy, and relation to infections): RMM (1994) 5 151162.]
The other species include e.g. S. acidominimus, S. bovis,
S. equinus and S. suis. Most of these species occur in domestic
animals (although e.g. S. bovis is an infrequent cause of
endocarditis in man).
A number of organisms, previously classified as streptococci,
have been transferred to the genera ENTEROCOCCUS and LACTOCOCCUS. (See also ATOPOBIUM.)
In addition to the three main groups of species (mentioned
above), many streptococci have been classified by LANCEFIELDS
STREPTOCOCCAL GROUPING TEST which identifies certain groupspecific cell-wall compounds; thus, e.g. species in the pyogenic group (see above) include those in Lancefield group A
(S. pyogenes), B (S. agalactiae), C (strains of S. dysgalactiae)
and G (S. canis). Note that the cell wall in some species does
741
Streptococcus
Some strains of S. pneumoniae form products such as
and THIOL-ACTIVATED CYTO-
streptomycin
sites on red blood cells (RBCs) and then oligomerize into ringshaped structures which form pores of 30 nm (larger than
the pores formed e.g. by the MAC in COMPLEMENT FIXATION).
Haemolysis is inhibited by free cholesterol.
Streptolysin O is immunogenic (cf. STREPTOLYSIN S), and it
cross-reacts with the theta toxin of Clostridium perfringens. In
certain diseases (e.g. RHEUMATIC FEVER) the titre of antistreptolysin O antibodies is typically elevated (see ANTISTREPTOLYSIN
O TEST).
[Mechanism of assembly of the streptolysin O pore: EMBO
(1998) 17 15981605.]
streptolysin S An oxygen-stable, non-immunogenic leucocidin
and haemolysin produced e.g. by many group A streptococci
(cf. STREPTOLYSIN O); it appears that some streptolysin S may
remain cell-bound while the rest is released by the cell. The
haemolytic activity of streptolysin S is inhibited by low levels
of certain phosphatides, e.g. phosphatidylethanolamine.
Streptomyces A genus of Gram-positive, aerobic bacteria (order
ACTINOMYCETALES, wall type I) which occur e.g. in soil and
aquatic habitats a few species being pathogenic in plants
(e.g. potato, sugar beet) and man (see MADUROMYCOSIS). The
organisms form both AERIAL MYCELIUM and a non-fragmenting,
branched SUBSTRATE MYCELIUM, and in most species spores
are formed only by the aerial mycelium which fragments to
give rise to non-verticillate chains of spores [differentiation
and spore formation: Book ref. 67, pp. 89115]; the genus
includes organisms which have been referred to as species of
Actinopycnidium, Actinosporangium and Chainia, and the genus
definition has been widened to include Elytrosporangium and
Microellobosporia (organisms which form spores on both substrate and aerial mycelium) [Book ref. 73, pp. 94105; JGM
(1983) 129 17431813]. (cf. STREPTOMYCETE.) The organisms
are chemoorganotrophic (metabolism: oxidative) and are not
nutritionally fastidious; usable carbon sources include e.g. chitin,
glucose, lactate, starch. Colonies are typically coloured, and
many species form a diffusible pigment. ANTIBIOTIC production
is common: see e.g. CARBAPENEMS, CHLORAMPHENICOL, CLAVULANIC ACID, MACROLIDE ANTIBIOTICS and STREPTOMYCIN. [Book
ref. 201.] (See also COMPLESTATIN.) GC%: 6978. Type species:
S. albus.
Studies on the cell envelope of S. griseus have revealed the
presence of a hydrophilic channel that runs through the cell wall,
and have further identified a streptomycin-binding site within the
channel [Mol. Microbiol. (2001) 41 665673].
Many of the hundreds of named species of Streptomyces have
been amalgamated to form a much smaller number of species
[see e.g. JGM (1983) 129 17431813]. [Ecology, isolation and
cultivation of streptomycetes: Book ref. 46, pp. 20282090.]
streptomycete Any organism of the (related) genera Intrasporangium, Kineosporia, Nocardioides, Sporichthya, Streptomyces
and Streptoverticillium [Book ref. 73, pp. 94105].
streptomycin A broad-spectrum AMINOGLYCOSIDE ANTIBIOTIC
produced by Streptomyces griseus; it consists of the base STREPTIDINE linked glycosidically to STREPTOBIOSAMINE. Streptomycin
is active against e.g. Mycobacterium tuberculosis, some staphylococci, Brucella spp and many other Gram-negative bacteria
(including some strains of Pseudomonas aeruginosa); bactericidal activity increases with concentration. The antibiotic is less
active, or inactive, under anaerobic conditions. Streptomycin also
inhibits vegetative growth and sporulation of certain fungi [JGM
(1983) 129 34013410].
When used as a chemotherapeutic agent, streptomycin is
associated with certain side-effects, including dose-dependent
streptonigrin
stress fibre See PINOCYTOSIS.
stretch-activated channel See MECHANOSENSITIVE CHANNEL.
Striaria See PHAEOPHYTA.
Striatella See DIATOMS.
strict (1) Syn. OBLIGATE. (2) A term used to emphasize the extent
to which a given term is applicable. For example, a strict
anaerobe is an organism which grows only in the complete
absence of oxygen (and which may also require a pre-reduced
medium), and strict anaerobiosis refers to the condition in
which there is a complete absence of oxygen. Similarly, a strict
autotroph can grow in the complete absence of organic carbon,
i.e. its carbon requirements can be satisfied by CO2 alone.
Strigomonas Syn. CRITHIDIA.
Strigula See CEPHALEUROS.
string of pearls effect See BACILLUS (B. anthracis).
stringency (in PCR) See PCR.
stringent control (1) (of rRNA and protein synthesis) In bacteria:
a control mechanism in which cells lacking an essential amino
acid respond with e.g. decreased synthesis of rRNA and proteins.
The response is triggered by an uncharged tRNA at a ribosomal
A site (see PROTEIN SYNTHESIS); this stimulates a ribosomebound enzyme, pyrophosphotransferase (RelA; the relA gene
product; stringent factor), to synthesize ppGpp (in which G
is guanosine, p is phosphate) from GTP (or GDP) and ATP.
ppGpp (= guanosine 5 -diphosphate 3 -diphosphate; guanosine
tetraphosphate) is an example of an ALARMONE. (Cells with a
null mutation in relA do not exhibit the stringent response and
are said to be relaxed.)
ppGpp can apparently enhance transcription from certain
operons that control the synthesis of particular amino acids (e.g.
histidine). ppGpp may thus help to maintain a correct balance of
amino acids in the cell; for example, given a level of histidine
low enough to trigger the stringent response, increased synthesis
of ppGpp may help to restore the balance by (i) slowing down
protein synthesis, and (ii) stimulating the his operon.
A high-resolution study revealed that ppGpp can bind to RNA
polymerase in different orientations. This suggested that basepairing between ppGpp and cytosines in non-template DNA
might be important in transcriptional control by ppGpp [Cell
(2004) 117 299310].
(2) (of plasmid replication) See PLASMID.
stringent factor See STRINGENT CONTROL (sense 1).
stripe rust Syn. YELLOW RUST.
stroma (1) (mycol.) A compact mass of prosenchymatous or
pseudoparenchymatous fungal tissue (or of intermingled fungal
and non-fungal tissue) on or within which spore-bearing or
spore-containing structures often develop. Stromata are formed
by many fungi e.g. by species of Nectria and Xylaria. (See
also ASCOSTROMA, SCLEROTIUM, SPORODOCHIUM.)
(2) See CHLOROPLAST.
stromatolites Rock-like accretions, often columnar or domed,
generally believed to have been formed by the incorporation
of sediment and/or precipitated calcareous/siliceous material in
MICROBIAL MATS within marine and non-marine habitats; the
oldest of such organosedimentary structures, ca. 3.5 109
years old, occur in Western Australia.
Stromatolites commonly exhibit a laminar (i.e. stratified)
pattern of construction; some authors use the term thrombolite
for analogous, non-laminar structures.
Calcified stromatolites apparently do not yield fossil microorganisms; however, cyanobacterium-like microfossils have been
detected in silicified stromatolites such organisms including
filaments (e.g. Gunflintia minuta) and coccoid organisms (e.g.
Huroniospora microreticulata). [Book ref. 154.]
subhymenium
and a long, non-contractile tail. Type species: BACTERIOPHAGE l
(q.v.). Other members: e.g., ACTINOPHAGES fC, R1, R2 and VP5;
Bacillus phages BPB1, f105 (q.v.), SPb and SPP1; Caulobacter crescentus phage fCbK; enterobacterial phages c (a FLAGELLOTROPIC PHAGE), PA2, f80, fD328, and T5; Pseudomonas
phage F116 (q.v.). Possible member: (virulent) coliphage T1.
(cf. LAMBDOID PHAGES.)
stylovirus A member of the STYLOVIRIDAE.
subacute bacterial endocarditis See ENDOCARDITIS.
subacute sclerosing panencephalitis (SSPE) An uncommon
disease of children and adolescents associated with persistent
measles virus (MV) infection (see MORBILLIVIRUS). Symptoms
begin insidiously, with intellectual deterioration and memory
loss followed by convulsions, spasticity, coma and death. MV
nucleocapsids can be detected as inclusion bodies in CNS
tissues, but budding viruses and infectious virions usually
cannot be detected. Persistence apparently involves defective
MV gene expression which may lead e.g. to a defect in MV
maturation. It is frequently associated with the absence or
reduced amounts of the virion M protein and/or with loss of
haemadsorption possibly resulting from M protein instability
and failure to process the H protein, respectively [Virol. (1985)
143 536545]. [Altered transcription of a defective MV genome
derived from a case of SSPE: EMBO (1987) 6 681688.]
SSPE viruses have been propagated by co-culture of infected
brain cells with e.g. Vero cells or human embryonic lung
cells. [Neurovirulence of cultured SSPE virus: JGV (1985) 66
373377.]
subacute spongiform encephalopathies (SSEs) The former
name for PRION-mediated diseases which are now referred to
as TRANSMISSIBLE SPONGIFORM ENCEPHALOPATHIES.
subclinical infection (med.) INFECTION (sense 2) in which symptoms are not apparent or the stage before symptoms become
apparent.
subculture (1) A CULTURE prepared by inoculating a medium
from an existing culture (cf. PRIMARY CULTURE). (2) The process
of preparing a culture as in (1). (3) (verb) To prepare a culture
as in (1).
suberin An aromatic polymer, somewhat similar to LIGNIN, to
which are attached (by ester linkages) aliphatic components, e.g.
!-hydroxy acids, dicarboxylic acids, C20 C30 alcohols. Suberin
occurs, with waxes, in the cell walls of underground parts of
higher plants, and is deposited e.g. at wound sites. (cf. CUTIN.)
It provides protection against infection etc, but the cutinases of
certain plant-pathogenic fungi may have some action on suberin.
[Book ref. 58, pp. 79100.]
suberization The deposition of SUBERIN by a plant e.g. at a site
of injury caused by fungi, insects etc.
suberosis An EXTRINSIC ALLERGIC ALVEOLITIS associated with
inhalation of cork dust contaminated with Penicillium frequentans.
subgenomic mRNA Of an RNA virus: an mRNA, produced
in an infected (eukaryotic) cell, which is shorter than the
genomic RNA. In eukaryotic cells, translation generally cannot
be initiated from an internal site in an mRNA strand; the
formation of a subgenomic mRNA allows an initiation site
which is located internally in the viral genome to be located
terminally, thus permitting independent translation of genes
within the genome (cf. POLYPROTEIN). Subgenomic mRNAs may
be monocistronic or polycistronic. (See e.g. CORONAVIRIDAE,
RETROVIRIDAE, TOBACCO MOSAIC VIRUS, TOGAVIRIDAE; cf. e.g.
FLAVIVIRIDAE.)
subhymenium Generative tissue immediately underlying a HYMENIUM. (See also APOTHECIUM.)
subiculum
dependent on Ca2+ for stability. [Production and properties:
Book ref. 31, pp. 5769.]
subtilysin Syn. SURFACTIN.
subviral agents Acellular infectious agents which lack one
or more of the essential features of a VIRUS; such agents
include SATELLITE RNAS, VIROIDS, VIRUSOIDS, PRIONS and the
(hypothetical) VIRINOS.
subviral particle A particle formed by certain viruses as an
intermediate in the replication cycle which consists of the
virion minus certain of its components (see e.g. REOVIRUS and
BACTERIOPHAGE f6).
succinate thiokinase See Appendix II(a).
Succinimonas A genus of Gram-negative bacteria (family BACTEROIDACEAE) which occur e.g. in the RUMEN. Cells: coccobacilli
or short rods, 1.01.5 1.03.0 m, which are monotrichously
(polarly) flagellated. Glucose, maltose or e.g. dextrins or starch
can be fermented; succinate and acetate are major products of
glucose fermentation. Fermentation is anaerogenic, and butyrate
is not formed. Type species: S. amylolytica.
Succinivibrio A genus of Gram-negative bacteria (family BACTEROIDACEAE) which occur e.g. in the RUMEN. Cells (when
freshly isolated): curved or helical rods, 0.40.6 1.07.0 m,
with pointed ends; monotrichously (polarly) flagellated. The
main products of glucose metabolism include succinate, acetate
and formate; glucose fermentation occurs anaerogenically, and
butyrate is not formed. The type species, S. dextrinosolvens,
appears to be a major fermenter of dextrins in ruminants fed
on high-starch diets.
succinylsulphathiazole See SULPHONAMIDES.
sucrase Syn. INVERTASE.
sucrose A non-reducing disaccharide: a-D-glucopyranosyl-b-Dfructofuranoside. It is produced by almost all photosynthetic
eukaryotes (but not by e.g. some diatoms and some red and green
algae). Sucrose can be metabolized by a range of microorganisms. Certain bacteria (e.g. Leuconostoc spp, Streptococcus spp)
split sucrose into its constituent monosaccharides, one of which
is metabolized while the other is polymerized to form DEXTRAN
or levan (see FRUCTANS). (See also INVERTASE.) High concentrations of sucrose can inhibit microorganisms and are used e.g. in
FOOD PRESERVATION.
Suctoria A subclass of freshwater and marine ciliates (class
KINETOFRAGMINOPHOREA) in which the adult cells are characteristically sedentary (commonly on a non-contractile stalk), lack
cilia (though they generally contain an infraciliature), and generally have few to many haptocyst-bearing tentacles. Prey organisms are ingested at the tips of the tentacles. Reproduction occurs
by budding, typically with the formation of motile, ciliated larval forms which lack tentacles. (See also BROOD POUCH.) Some
species are loricate. Genera include e.g. Acineta, Dactylostoma,
Dendrosoma, Podophrya, Sphaerophrya, and Tokophyra. (See
also PHALACROCLEPTES.)
suctorian A ciliate of the subclass SUCTORIA.
Sudan black B A blue-black diazo LYSOCHROME used (0.3% w/v
in 70% ethanol) for staining intracellular lipid: see BURDONS
STAIN.
sudanophilic Having an affinity for lipid stains (e.g. SUDAN
BLACK B).
sudden infant death syndrome (SIDS; syn. cot death, crib death)
The sudden death of an infant (typically aged between ca. 3
weeks and 5 months) with no apparent cause. Various infections
have been implicated as causes of SIDS, including e.g. rotavirus
infection [JMV (1982) 10 291296] and BOTULISM, but often
there is no evidence of microbial involvement.
sulphate-reducing bacteria
Sudol See PHENOLS.
suffocation disease A disease of the rice plant which is apparently due to toxic levels of hydrogen sulphide produced by
microorganisms in the flooded soils used for rice cultivation.
Plants may be protected from sulphide by the activities of
sulphide-utilizing microorganisms (e.g. Beggiatoa). (See also
CEREAL DISEASES and SULPHATE-REDUCING BACTERIA.)
sufu A Chinese fermented soybean food resembling soft cream
cheese. Soybeans are ground, boiled or steamed, strained, and
a coagulant (e.g. CaSO4 , MgSO4 , acetic acid) is added to the
liquid fraction to precipitate proteins. The precipitate is pressed
to form a cubical cake-like curd (tofu), surface-inoculated with
a fungus (e.g. Actinomucor elegans, Mucor spp), and incubated
at e.g. 20 C for 37 days. The cubes are salted, rinsed, and
immersed in brine containing alcohol, flavouring etc, and aged
for e.g. 13 months. [Book ref. 8, pp. 516520.]
sugar alcohol See POLYOL.
sugar beet yellows virus (SBYV) The type member of the
CLOSTEROVIRUSES. SBYV can infect a wide range of plants; in
sugar beet, symptoms include yellowing and necrosis spreading
inwards from the leaf tips and margins.
sugarcane diseases Diseases of sugarcane (Saccharum officinarum) include e.g. FIJI DISEASE and RED ROT. [Details of various
sugarcane diseases classified according to causal agent: Phytopathol. Paper number 29, February 1986.]
sugarcane Fiji disease virus See FIJIVIRUS.
sugarcane mosaic virus See POTYVIRUSES.
sugars See PEPTONE-WATER SUGARS.
suicide gene Any gene whose expression in a cell is lethal for
that cell.
suicide substrate Any substrate whose uptake or metabolism by
a cell is lethal for that cell.
suid (alpha) herpesvirus 1 See ALPHAHERPESVIRINAE.
suid herpesvirus 1 group See ALPHAHERPESVIRINAE.
suid herpesvirus 2 See BETAHERPESVIRINAE.
Suipoxvirus (swinepox subgroup)
A genus of viruses of the
CHORDOPOXVIRINAE; the genus includes the swinepox virus (see
SWINE POX).
sulA gene See SOS SYSTEM.
sulB gene See SOS SYSTEM.
sulbactam A b-LACTAMASE INHIBITOR. (See also SULTAMICILLIN.)
sulconazole See AZOLE ANTIFUNGAL AGENTS.
sulcus A groove: see e.g. DINOFLAGELLATES.
sulfate- See sulphate-.
sulfazecin See MONOBACTAMS.
Sulfolobus A genus of thermophilic, aerobic and facultatively
anaerobic sulphur-dependent prokaryotes (domain ARCHAEA, formerly Archaebacteria) which occur e.g. in certain hot springs
(see also COAL BIODEGRADATION). Cells: cocci, coccoid or irregularly shaped forms; the CELL WALL is an S LAYER. Growth occurs
between ca. 50 and 90 C, at pH ca. 15. Many strains are
facultatively CHEMOLITHOAUTOTROPHIC (q.v.), but some are obligately heterotrophic. Energy is obtained by the oxidation of
sulphur (or Fe2+ ) and/or by SULPHUR RESPIRATION. CO2 is assimilated via a reductive tricarboxylic acid pathway. Species include
S. acidocaldarius, S. ambivalens and S. solfataricus. (See also
REVERSE GYRASE and SULPHUR CYCLE.)
sulfur- See sulphur-.
sulpha drugs (1) Syn. SULPHONAMIDES. (2) The sulphonamides
and the SULPHONES.
sulphacetamide See SULPHONAMIDES.
sulphadiazine 4-Amino-N-2-pyrimidinylbenzenesulphonamide:
one of the more effective and less toxic of the antibacterial
SULPHONAMIDES; it is rapidly absorbed from the gut, and is effective against e.g. streptococci, Neisseria spp, Escherichia coli,
etc. Sodium sulphadiazine may be given intravenously e.g. in
the treatment of meningococcal meningitis; silver sulphadiazine
(see SILVER) is used topically in the treatment of burns.
sulphadimethoxine See SULPHONAMIDES.
sulphadimidine See SULPHONAMIDES.
sulphadoxine A SULPHONAMIDE which has been used (e.g. in
combination with pyrimethamine) for the treatment of clinically uncomplicated, chloroquine-resistant MALARIA. Sulphadoxine and pyrimethamine act synergistically to block (i) the synthesis of dihydrofolate (DHF) and (ii) the reduction of DHF to
tetrahydrofolate (THF). Resistance to sulphadoxine may arise
through the effects of mutation on the target enzyme [Eur. J.
Bioch. (1994) 224 397405].
sulphaguanidine See SULPHONAMIDES.
sulphamethazine See SULPHONAMIDES.
sulphamethizole See SULPHONAMIDES.
sulphamethoxazole See SULPHONAMIDES.
sulphamylon Syn. MARFANIL.
sulphanilamide See SULPHONAMIDES.
sulphate assimilation See ASSIMILATORY SULPHATE REDUCTION.
sulphate-reducing bacteria A phrase traditionally used to refer
to a (non-taxonomic) category of strictly anaerobic bacteria
which are characterized by their ability to carry out DISSIMILATORY SULPHATE REDUCTION. The organisms include cocci, rods
and filaments, most stain Gram-negatively, and the cells of one
genus (DESULFOTOMACULUM) form endospores. They occur e.g.
in soil; in anaerobic muds and sediments in freshwater, brackish
and marine habitats; in the RUMEN, and in the intestinal tract in
man and other animals; and in sewage. Some species tolerate or
need salt (NaCl); the spore-forming sulphate-reducing bacteria
tolerate a maximum of ca. 2% NaCl. In vitro culture requires
the use of pre-reduced media in which the REDOX POTENTIAL is
more negative than ca. 100 mV.
Substrates used as electron donors include e.g. lactate, propionate, pyruvate and certain alcohols; according to species these
may be oxidized to acetate and CO2 or (completely) to CO2 .
[Use of amino acids as energy substrates by marine strains of
Desulfovibrio: FEMS Ecol. (1985) 31 1115.] Electron acceptors include sulphate, sulphite (see also DESULFOVIRIDIN), thiosulphate and tetrathionate; such oxidized compounds of sulphur
may be derived from biological activity (see e.g. SULPHURETUM)
or from the autoxidation of sulphide [FEMS Ecol. (1985) 31
3945]. At least some strains can use nitrate and/or fumarate as
electron acceptors instead of oxidized sulphur compounds.
Some strains can grow mixotrophically by oxidizing H2 (see
e.g. DESULFOVIBRIO), some can gain energy from pyrophosphate
(see DESULFOTOMACULUM), and many can derive energy from
pyruvate via the PHOSPHOROCLASTIC SPLIT. In the absence of an
oxidized sulphur compound some species exhibit fermentative
metabolism, although carbohydrates are rarely used. (See also
FERMENTATION sense 1.)
The activities of the sulphate-reducing bacteria are responsible
for much of the H2 S produced in organically polluted waters.
In rice paddies H2 S can be beneficial (e.g. by killing parasitic
nematodes) but high concentrations of H2 S are phytotoxic
and can damage crops (see also SUFFOCATION DISEASE); nitrate
(which inhibits sulphate reduction) has been used to control this
problem. Sulphide from these bacteria is often at least partly
responsible for the corrosion of underground ferrous pipes (see
also CATHODIC DEPOLARIZATION THEORY and TUBERCLE (sense 2))
and for the degeneration of concrete and stonework; metals
747
sulphate reduction
can be affected by the sulphide itself, but damage to concrete
and stone derives primarily from the action of sulphuric acid
produced from the sulphide by e.g. thiobacilli.
[Microbial sulphate reduction in the early Archaean era:
Nature (2001) 410 7781.]
(See also DESULFOBACTER, DESULFOBULBUS, DESULFOCOCCUS,
DESULFOTOMACULUM, DESULFOMONAS, DESULFONEMA, DESULFOSARCINA, DESULFOVIBRIO.)
[Book ref. 102.]
sulphate reduction The microbial reduction of sulphate may
involve ASSIMILATORY SULPHATE REDUCTION or DISSIMILATORY
SULPHATE REDUCTION. (See also SULPHUR CYCLE.)
sulphate respiration Syn. DISSIMILATORY SULPHATE REDUCTION.
sulphathiazole See SULPHONAMIDES.
sulphide See HYDROGEN SULPHIDE.
sulphite fermentation See NEUBERGS FERMENTATIONS.
sulphonamides A group of chemotherapeutic agents. The antimicrobial sulphonamides are mostly derivatives of sulphanilamide
(p-aminobenzenesulphonamide: NH2 .C6 H4 .SO2 .NH2 ) (cf. MARFANIL); they are microbistatic for a wide range of Gram-positive
and Gram-negative bacteria, and for various protozoa (e.g. coccidia, Plasmodium spp). Sulphonamides are used usually in
combination with other chemotherapeutic agents (see e.g. FOLIC
ACID ANTAGONISTS) for treating certain urinary tract infections,
MALARIA (q.v.), coccidioses, etc.
Sulphonamides act as structural analogues of p-aminobenzoic
acid (PABA), competitively inhibiting the incorporation of
PABA during the formation of dihydropteroic acid in FOLIC
ACID synthesis. Those organisms which synthesize their own
folic acid and which cannot use an exogenous supply of the
vitamin are sensitive to sulphonamides (provided that the cells
are permeable to the drugs), while organisms which require
exogenous folic acid for growth are insensitive. A lag period of
several generations occurs between exposure of sensitive cells to
sulphonamide and growth inhibition; during this time the cells
exhaust their pre-formed supply of endogenous folic acid. This
delayed effect allows sulphonamides to be used in combination
with antibiotics (e.g. penicillins) which are active only against
growing organisms.
The inhibitory effect of sulphonamides may be neutralized
by supplying the cells with those metabolites which normally
require folic acid for their synthesis (e.g. purines, certain amino
acids); such substances may be present e.g. in pus, so that
sulphonamides may be ineffective in the treatment of certain
suppurative infections. Bacteria readily develop resistance to
sulphonamides: e.g., in Streptococcus pneumoniae modification
of dihydropteroic acid synthetase by a single-step mutation may
reduce the affinity of the enzyme for sulphonamides without
significantly reducing its affinity for PABA. Plasmid-borne
resistance also occurs, and can involve e.g. a plasmid-encoded
sulphonamide-resistant dihydropteroic acid synthetase. (See also
entries Tn21 and Tn2410.)
The many sulphonamides differ e.g. in their clinical properties, toxicities, etc. Most are derivatives bearing substituents at
the nitrogen of the sulphonamide group (NH2 .C6 H4 .SO2 .NHR).
Substitution at the p-amino group results in the loss of antibacterial activity; however, such derivatives may be hydrolysed in vivo to an active derivative. For example, p-Nsuccinylsulphathiazole and phthalylsulphathiazole are inactive
and are poorly absorbed from the gut, but they are hydrolysed
in the lower intestine to release the active component sulphathiazole; these drugs have been used e.g. pre- and post-operatively
in abdominal surgery.
Sulphonamides include e.g. sulphacetamide (N-[(4-aminophenyl)sulphonyl]-acetamide); SULPHADIAZINE; sulphadimethoxine (4-amino-N-(2,6-dimethoxy-4-pyrimidinyl)benzenesulphonamide); sulphadimidine (= sulphamethazine: 4-amino-N(4,6-dimethyl-2-pyrimidinyl)benzenesulphonamide); sulphaguanidine (4-amino-N-(aminoiminomethyl)benzenesulphonamide);
sulphamethizole (4-amino-N-(5-methyl-1,3,4-thiadiazol-2-yl)
benzenesulphonamide); sulphamethoxazole (4-amino-N-(5methyl-3-isoxazolyl)benzenesulphonamide); sulphathiazole (4amino-N-2-thiazolylbenzenesulphonamide); etc.
(See also PAS; PRONTOSIL; SULPHONES.)
sulphonation See WATER SUPPLIES.
sulphones Antibacterial agents (general formula: R2 SO2 ) active
against a range of species; owing to toxicity they are not widely
used in medicine. An example is DAPSONE.
sulphorhodamine 101 acid chloride See TEXAS RED.
sulphorhodamine B See LISSAMINE RHODAMINE.
sulphur (as an ANTIFUNGAL AGENT) Elemental sulphur is generally effective against certain plant diseases of fungal aetiology,
e.g., apple scab, powdery mildews, black spot of roses; it may
be applied as a fine dust, as a WETTABLE POWDER, or in colloidal
form. The degree of fungitoxicity is related to the size of the
sulphur particles, the smallest particles generally being the most
toxic.
Sulphur may be applied as polysulphide: a product (formed
by the reaction of certain metal sulphides with sulphur under
alkaline conditions) which, when acidified e.g. by atmospheric
CO2 , liberates elemental sulphur. An early preparation, liver
of sulphur (potassium polysulphide), was made by the fusion
of potassium hydroxide and sulphur. Lime sulphur is prepared
by boiling sulphur with lime the resulting solution containing
calcium thiosulphate and calcium polysulphide; it tends to be
phytotoxic and is incompatible with many chemical pesticides
owing to its alkalinity. Green sulphur contains finely divided
sulphur and certain iron compounds; it is formed as a by-product
of a coal-gas purification process in which hydrogen sulphide
reacts with ferric oxide.
Elemental sulphur can cause premature defoliation and dropping of fruit in certain varieties of fruit tree a phenomenon
called sulphur shyness.
sulphur bacteria Those bacteria which contribute to stage(s)
of the SULPHUR CYCLE other than assimilatory sulphate reduction and the decomposition of organic sulphur compounds to
sulphide; they include the SULPHATE-REDUCING BACTERIA, certain photosynthetic bacteria, and species/strains of Beggiatoa,
Desulfuromonas, Oscillatoria and Thiobacillus. (cf. COLOURLESS
SULPHUR BACTERIA.) [Biochemistry and ecology of the sulphur
bacteria: PTRSLB (1982) 298 429602.]
(See also SULPHUR-DEPENDENT ARCHAEANS.)
sulphur cycle In nature: the cyclical interconversion of sulphur
and its compounds. The figure shows some of the interconversions carried out by bacteria (see also SULPHUR-DEPENDENT
ARCHAEANS).
In addition to biological interconversions, sulphide can be
oxidized by autoxidation [see e.g. FEMS Ecol. (1985) 31
3945] to e.g. elemental sulphur, thiosulphate and sulphate.
Sulphur is required e.g. for the synthesis of certain amino
acids, ferredoxins and cofactors such as coenzyme A. Many
bacteria assimilate sulphur in the form of sulphate which is
usually available in adequate quantities in the environment;
the sulphate is initially reduced to sulphide (see ASSIMILATORY
SULPHATE REDUCTION).
748
sulphur dioxide
SO 4
su
ss
lph
im
ate
ila
n
tio
re
sp
ira
n
tio
Thiobacillus ferrooxidans
Thiobacillus thiooxidans
sulphate-reducing
bacteria
SO 3
Rhodopseudomonas
sulfidophila
SO 3
hate r
ed
organic
sulphur
s u lp
Thiobacillus
or y
ila t
as
s im
on
s im
ilati
as
mine
rali
zat
ion
Desulfuromonas
h
sulp
uction
elemental
sulphur
ate
p
res
sulphate-reducing
bacteria
i ra
ti o
SULPHUR CYCLE: some interconversions carried out by bacteria. Many species can use sulphate as a source of sulphur (shown here as
assimilatory sulphate reduction). The sulphate is reduced, intracellularly, to sulphide, and the sulphide is incorporated in different ways by
different species; in e.g. Escherichia coli, sulphide is incorporated into O-acetylserine to form cysteine.
In a dissimilatory mode, sulphate respiration is carried out e.g. by the sulphate-reducing bacteria sulphate being used as terminal electron
acceptor in anaerobic respiration. Elemental sulphur is used as terminal electron acceptor by Desulfuromonas. Thiobacillus spp carry out
aerobic respiration in which e.g. sulphide or elemental sulphur is oxidized. Rhodopseudomonas sulfidophila is one of a number of species
which use sulphide as an electron donor in anaerobic phototrophic metabolism.
Reproduced from Bacteria 5th edition, Figure 10.3, page 262, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471-98880-4)
with permission from the publisher.
BACTERIA; SULPHUR-REDUCING BACTERIA; SULPHURETUM; THIOBA-
CILLUS.
sulphur granules
that expresses a particular Vb chain (see T CELL RECEPTOR),
and (ii) an MHC class II molecule on an antigen-presenting
cell (e.g. a macrophage or B cell); such binding, in which the
superantigen acts as a cross-link between the Vb chain and the
class II molecule, causes (i) T cell proliferation, and (ii) release
of cytokines from the T cell and from the antigen-presenting
cell. Because many different strains of T cell express a given Vb
chain, a superantigen causes polyclonal activation of T cells (as
though the corresponding range of antigens had been present);
this is accompanied by a massive release of cytokines. During
the joint stimulation of a T cell and a macrophage, the cytokines
released include IL-1, IL-2, IL-4, IL-6, IL-8, TNF-a, TNF-b and
IFN-g.
Superantigens are able to activate both CD4+ and CD8+
cells, binding to the Vb chain at a site outside the normal
antigen-binding region. Activation and proliferation of T cells
naturally gives rise to an initial increase in the number of T
cells of the given Vb subset; however, there is evidence to
suggest that many of the T cells which bind superantigen either
become unresponsive (= T cell anergy) or undergo apoptosis.
Thus, while the T cell population of a given subset may initially
rise, there may be a net loss of functional cells of that subset in
the longer term.
Superantigens include the five major ENTEROTOXINS of Staphylococcus aureus (SEA, SEB, SEC, SED and SEE), the toxic
shock syndrome toxin 1 (TSST-1; formerly enterotoxin F)
of S. aureus, and the exotoxin A of Streptococcus pyogenes
(= streptococcal superantigen A; SSA). Different superantigens
bind preferentially to different Vb chains; for example, TSST-1
binds to Vb type 2, SED binds to Vb 5 and 12, and SEA binds
to Vb types 1, 5, 6, 7 and 9.
Superantigens are apparently associated with some viruses,
e.g. rabies virus.
The ability of a superantigen to induce massive release of
cytokines is apparently involved in the pathogenesis of TOXIC
SHOCK SYNDROME. It has been suggested that this mechanism
may also be responsible for at least some of the symptoms of
certain other diseases (such as KAWASAKI DISEASE).
B cell superantigens are analogous molecules; they bind to
the VH chain of the B cell receptor.
[Clinical significance of T cell superantigens: TIM (1998) 6
6165.]
superchlorination See WATER SUPPLIES.
supercoiled DNA See DNA.
supercoiling-induced duplex destabilization See SIDD.
superelongation disease (of cassava) See GIBBERELLINS.
superhelical DNA See DNA.
superhelix density (s) See DNA.
superhelix winding number (t) See DNA.
superinfection exclusion See SUPERINFECTION IMMUNITY.
superinfection immunity A phenomenon in which a virusinfected cell can resist infection by a second virus of the same
or a similar type. The second virus may be prevented from
adsorbing to or penetrating the cell (superinfection exclusion),
or it may enter the cell but be unable to replicate. For example,
if a bacterial cell contains a l prophage (see LYSOGENY), any
incoming l genome will immediately be subject to repression by
the repressor encoded by the incumbent prophage. When phage
P22 establishes a lysogenic infection in Salmonella typhimurium,
it causes glycosylation of the LPS of the host cell, resulting
in modification of the P22 receptor sites and preventing further
infection by P22. These are examples of lysogenic (or prophage)
immunity; superinfection immunity may also be exhibited by
lytic phages such as T4. (See also e.g. RETROVIRIDAE.)
suppressor mutation
Phages which belong to the same immunity group (i.e., one
cannot infect a cell already infected by any of the others in the
group) are said to be homoimmune; phages of different immunity
groups are said to be heteroimmune. (See e.g. LAMBDOID PHAGES.)
(The term superinfection immunity has also been applied to
some cases of INCOMPATIBILITY in plasmids.)
superoxide (superoxide radical) A term used to refer either to
periplasmic (sodB-encoded) FeSOD and an inducible, cytoplasmic (sodA-encoded) MnSOD the intracellular concentration of
superoxide anion appears not to regulate the oxygen-dependent
synthesis of the MnSOD [PNAS (1984) 81 49704973].
In Lactobacillus plantarum (in which SODs are absent) the
is carried out by manganese a metal
dismutation of O
2
accumulated to an intracellular concentration of ca. 25 mM; the
low efficiency of manganese as a dismutase appears to be offset
by its high intracellular concentration. (L. plantarum becomes
oxygen-sensitive in manganese-deficient media.) Certain other
organisms (e.g. Mycoplasma pneumoniae [BBRC (1980) 96
98105]) lack SODs but their functional equivalent(s) (if any)
are unknown.
[Varieties, distribution, physiological functions of SODs:
ARPT (1983) 23 239257 (pp. 244249); SOD, an evolutionary puzzle: PNAS (1985) 82 824828; SOD mutants of
Escherichia coli: EMBO (1986) 5 623630.]
superoxide radical Syn. SUPEROXIDE.
superoxol test A form of CATALASE TEST in which 20% or 30%
H2 O2 is used in place of the more usual 3%. It may be used
e.g. in the presumptive identification of Neisseria gonorrhoeae
[BJVD (1984) 60 8789].
super-repressor See e.g. LAC OPERON.
supertwisted DNA Supercoiled DNA.
supervital staining See VITAL STAINING.
support film See ELECTRON MICROSCOPY (a).
suppressive petite See PETITE MUTANT.
suppressive soils Soils which suppress the survival, growth,
and/or pathogenic activity of particular plant-pathogenic fungi.
In at least some cases suppression is due to the presence of
an antagonistic microflora: e.g., mycophagous amoebae may
be involved in the suppression of TAKE-ALL [SBB (1984) 16
197199].
suppressor mutation (suppressor) A MUTATION which alleviates
the effects of a previous (primary) mutation at a different locus
(second-site reversion); commonly, the wild-type phenotype is
only partially restored, resulting in a pseudo-wild phenotype.
(cf. BACK MUTATION.)
In intragenic suppression, both primary and suppressor mutations occur in the same gene. For example: (a) A (primary)
MIS-SENSE MUTATION which results in an inactive gene product can be countered by a second (suppressor) mutation elsewhere in the same gene which allows the gene product to adopt
a conformation capable of at least some activity. (b) A primary
FRAMESHIFT MUTATION may be suppressed by a second nucleotide
deletion/insertion which restores the correct reading frame; the
nucleotide sequence between the two mutations will still be read
out of phase.
In intergenic suppression the suppressor mutation occurs
in a gene (designated sup) other than that containing the
primary mutation. A direct intergenic suppressor (informational
suppressor ) usually affects a tRNA molecule and results in
e.g. the insertion of an amino acid at the site of a nonsense
mutation (nonsense suppressor ) or a different amino acid at
the site of a mis-sense mutation (mis-sense suppressor ). The
activity of the resulting gene product will depend on the
suitability of the amino acid inserted. Various types of direct
intergenic suppressor are known. For example: (a) A mutation
in a tRNA gene may alter the anticodon of the tRNA such
that it recognizes a codon containing a nonsense mutation
or a mis-sense mutation. Thus, e.g., an ochre suppressor in
a gene for tRNAGln may alter the anticodon from NUG to
NUA (N = nucleotide), allowing the tRNA to recognize the
751
suppressor-sensitive mutation
Res. (1987) 7 110]; however, its potential in the treatment of
AIDS is probably limited [see e.g. AIM (1986) 105 3237].
surface electrophoresis See ELECTROPHORESIS.
surface exclusion (entry exclusion) The phenomenon in which
the presence of a conjugative plasmid in a cell reduces the
ability of that cell to receive an identical or related plasmid, by
CONJUGATION (sense 1b), from another cell. (cf. SUPERINFECTION
IMMUNITY.) In the Escherichia coli /F PLASMID conjugal system,
surface exclusion involves the products of genes traS (a
cytoplasmic membrane protein) and traT (an OUTER MEMBRANE
protein); the traT product appears to inhibit stable contact
between donor cells. The effect of surface exclusion may be
lost if e.g. donor cells progress to the stationary phase of growth
or are starved of amino acids; such cells, which can act as
recipients, are called F phenocopies. (Cells which express the
traT gene are, incidentally, less susceptible to PHAGOCYTOSIS and
to SERUM KILLING; resistance to serum killing apparently derives
from the ability of the TraT protein to inhibit the assembly
or action of the membrane attack complex (see COMPLEMENT
FIXATION) [JGM (1985) 131 15111521].)
An analogous effect appears to occur in cells of Enterococcus
faecalis carrying the conjugative plasmid pCF-10; when these
donor cells are exposed to recipient PHEROMONES they form a
cell-surface protein which inhibits their ability to act as recipients
for a derivative of pCF-10 [PNAS (1985) 82 85828586].
surface-obligatory conjugation system See PILI.
surface plasmon resonance See BIACORE.
surface-preferred conjugation system See PILI.
surfactin (subtilysin) A highly effective lipopeptide BIOSURFACTANT produced by Bacillus subtilis; it consists of a cyclic
heptapeptide covalently linked to a hydroxy fatty acid. Surfactin
is haemolytic and can also lyse the protoplasts of certain bacteria;
it is not immunogenic.
Surirella See DIATOMS.
surra A disease of e.g. camels and horses which occurs in
Africa (including Madagascar and Mauritius), Asia (e.g. India)
and South America (cf. MAL DE CADERAS); it is caused by Trypanosoma evansi and is transmitted non-cyclically by biting flies
(e.g. Stomoxys, Tabanus) or, in South America, by blood-sucking
vampire bats (Desmodus). (Various animals, e.g. buffaloes, cattle, deer, sheep, may act as reservoirs of infection.) Symptoms
include weakness, recurrent fever, and wasting; the disease is
often fatal. Lab. diagnosis: e.g. indirect fluorescent antibody and
haemagglutination tests. Treatment. In horses, the disease has
been treated with e.g. arsenicals (e.g. tryparsamide), while prophylaxis has been achieved e.g. with quinapyramine-SURAMIN
complexes.
surrogate light chains See B LYMPHOCYTE.
sus mutant A suppressor-sensitive (amber) mutant.
suspension test A test, used to determine the efficacy of a
DISINFECTANT, in which the disinfectant is allowed to act for
a specified time(s) on organisms suspended in a liquid medium
and/or diluent. (cf. CARRIER TEST.) In a qualitative suspension
test (e.g. the RIDEALWALKER TEST) the effect of the disinfectant
is determined by subculturing the test suspension to a liquid
growth medium to detect the presence of viable organisms; in
quantitative suspension tests (e.g., the FIVE-FIVE-FIVE TEST) the
effect of the disinfectant is determined by counting the viable
organisms remaining in the test suspension.
suspensor (mycol.) A clavate or conical structure formed by a
PROGAMETANGIUM. In some species (e.g. Phycomyces blakesleeanus) the suspensor gives rise to short filaments or spines.
suture (1) A line which marks the junction of two parts or
`
SECANT
.
structures. (2) (ciliate protozool.) See SYSTEME
swine erysipelas
suzukacillin See ALAMETHICIN.
SV40 SIMIAN VIRUS 40.
SVD SWINE VESICULAR DISEASE.
Svedberg unit (S) The unit in which the sedimentation coefficient
of a particle (e.g. a macromolecule) is commonly quoted. The
sedimentation coefficient (= sedimentation constant), s, is given
by:
dx 1
s=
dt !2 r
in which dx/dt is the measured sedimentation rate (in the
ultracentrifuge), ! is the angular velocity (radians sec1 ), and
r is the distance (cm) between a point within the sample and
the axis of rotation; when values are substituted in the above
expression, s is obtained in terms of reciprocal seconds. The
unit is the Svedberg unit (1013 sec).
swab (microbiol.) A device used for sampling the microflora at a
given site. Swabs suitable for laboratory or clinical use typically
consist of a compact piece of COTTON WOOL securely attached
to one end of a thin wooden stick or a piece of wire; a sterile
swab may be used for transferring material e.g. from the throat
to a bacteriological culture medium. (See also SPREAD PLATE.)
(Calcium ALGINATE wool may be used instead of cotton wool;
it dissolves in e.g. aqueous sodium citrate, or in 1% sodium
hexametaphosphate in quarter-strength Ringers solution thus
releasing all organisms trapped in its fibres.) (See also MOORE
SWAB.)
swamp cancer Syn. EQUINE PHYCOMYCOSIS.
swamp fever (equine infectious anaemia) An infectious HORSE
DISEASE caused by a retrovirus (generally considered to be
a member of the LENTIVIRINAE). Swamp fever occurs e.g. in
Europe, Canada and the USA. It is transmitted by biting flies
and mosquitoes. Incubation period: 24 weeks. The initial
stage of the disease is typically acute, with e.g. anaemia,
depression, incoordination, intermittent fever, myocarditis and
splenomegaly. Animals may recover temporarily (only to relapse
after 23 weeks with similar but usually less severe signs),
or they may become progressively weaker and die after ca.
1014 days. In survivors, relapses which apparently result
from ANTIGENIC VARIATION in virion surface glycoprotein may
continue to occur, and the animals probably remain carriers
for life; viraemia occurs even during remissions. The virus
replicates in and destroys host macrophages, and many of the
symptoms may result from the deposition of immune complexes.
Lab. diagnosis: e.g. an agar gel immunodiffusion test for serum
precipitins. Control: e.g. slaughter of infected animals. [Book
ref. 33, pp. 713717.]
swan animalcule The ciliate Lacrymaria olor.
swan-neck flask Apparatus used by Pasteur to refute the doctrine
of ABIOGENESIS. Each spherical glass flask had a long narrow
neck which was bent downwards then upwards, thus inhibiting
the access of airborne microorganisms to the sterilized contents
of the flask.
swarm (1) (verb) To exhibit SWARMING (sense 1 or 2). (2) (bacteriol.) A motile colony formed e.g. by gliding bacteria. (3) A
PSEUDOPLASMODIUM (sense 3).
swarm cell (1) Syn. SWARMER. (2) See e.g. SWARMING.
swarm period See e.g. DIPLANETISM.
swarm spores Motile spores.
swarmer (swarm cell) An actively motile cell which has developed from a non-motile precursor see e.g. CAULOBACTER,
RHODOMICROBIUM.
swarming (1) A phenomenon, involving morphological and
functional differentiation, exhibited when certain species of
swine fever
occurs via the mouth or wounds; it may lead to sudden death,
or symptoms may include e.g. fever, prostration, abortion, and
(pathognomonic) diamond-shaped skin lesions. Affected animals
may die, may recover (but remain carriers), or may develop
chronic disease with e.g. progressive unthriftiness, arthritis,
and valvular lesions in the heart. Treatment: e.g. penicillins.
Prophylaxis: e.g. vaccination.
E. rhusiopathiae can also cause erysipelas in poultry (particularly turkeys); the disease is commonly fatal. Birds may be
protected by vaccination.
swine fever (European swine fever; hog cholera) A highly infectious, mild or severe PIG DISEASE caused by a virus of the genus
Pestivirus (see TOGAVIRIDAE). Infection occurs via the mouth or
nose; the incubation period is usually ca. 510 days. In the acute
disease there is fever, lethargy, conjunctivitis with discharge, and
constipation followed by diarrhoea; reddish patches appear on
the skin, and there are signs of CNS involvement (convulsions,
circling, incoordination, ataxia). Haemorrhagic lesions of internal organs are found post mortem. Mortality rates may be high.
In the chronic disease (low-virulence virus) there may be transient fever with few other clinical signs; button ulcers (12 cm
diam.) may be found (mainly) in the large intestine post mortem.
The virus may cross the placenta and infect fetuses, causing
abortion or congenital tremor. (cf. AFRICAN SWINE FEVER.)
swine infertility and reproductive syndrome virus See BLUEEARED PIG DISEASE.
swine influenza A PIG DISEASE, affecting the respiratory tract,
apparently caused jointly by an influenza A virus (see INFLUENZAVIRUS) and Haemophilus parasuis [Book ref. 33, pp. 790791].
Symptoms: coughing, dyspnoea and prostration. Recovery is
usually rapid, but may be complicated by secondary infection
with e.g. Pasteurella multocida. Virus commonly persists in carrier pigs and can be carried e.g. by the lungworm Metastrongylus
apri.
swine pox A (usually benign) PIG DISEASE caused by a Suipoxvirus; typical vesicular pox lesions develop mainly on the
abdomen. Mortality rates may be high in suckling piglets. The
virus is commonly transmitted by the pig louse (Hematopinus
suis).
swine vesicular disease (SVD) An infectious PIG DISEASE clinically indistinguishable from FOOT AND MOUTH DISEASE (although
cattle and sheep are not affected); it occurs e.g. in Europe
and Japan. SVD is caused by a porcine ENTEROVIRUS. Infection occurs mainly via the tonsils, but also via the gut, wounds,
abrasions etc. Incubation period: 27 days; the mortality rate is
usually low. Transmission is mainly by pigpig contact; a carrier state is unknown. The virus can survive for months e.g. in
moist pig faeces; it is stable between pH 2.5 and 12, but can be
inactivated by moist heat (60 C/30 min).
swineherds disease LEPTOSPIROSIS caused by L. interrogans
serotype pomona.
swinepox subgroup See SUIPOXVIRUS.
Swiss cheeses See CHEESE-MAKING.
swivelase A type I TOPOISOMERASE.
SXT A combination of sulphamethoxazole and trimethoprim;
SXT-impregnated discs are used in an identification test for
streptococci b-haemolytic streptococci of Lancefield groups A
and B usually being resistant to SXT.
SYBR Green I See PCR.
Syc Specific Yop chaperone: see VIRULON.
Sydenhams chorea See RHEUMATIC FEVER.
Sym plasmid See ROOT NODULES.
Symba process See SINGLE-CELL PROTEIN.
Synechocystis
thymidine. Cells passing through the S phase of the CELL CYCLE
remain blocked in that phase, while all other cells continue their
development to the end of G1 . (Development beyond G1 does
not occur during the blockade.) The cells are then exposed to a
thymidine-free medium for a period of time equal to that of the S
phase; during this time all the cells continue their development,
and, at the end of the period, no cells are passing through
phase S. The cells are then re-exposed to excess thymidine until
all the cells have reached the end of G1 i.e., the culture has
become synchronous.
In a simpler, selective method for synchronization of mammalian cells, a tissue culture is gently agitated; cells undergoing mitosis are more easily detached from the glass, and can
be decanted with the growth medium, giving a suspension of
approximately synchronous M phase cells.
In the absence of a synchronizing influence, synchronous
cultures normally return to the asynchronous condition.
Synchytrium
A genus of unicellular, endobiotic, holocarpic
fungi (order CHYTRIDIALES) which are parasitic on various plants
(see e.g. WART DISEASE). The asexual cycle of S. endobioticum
resembles that of OLPIDIUM species except that e.g. each zoospore
may give rise to a group of sporangia (a sorus). Sexually-formed
thick-walled resting sporangia are also produced.
syncilium A group or tuft of cilia which resembles other forms
of COMPOUND CILIATURE but which differs in the infraciliary
organization; syncilia occur in the ENTODINIOMORPHIDA.
syncytium (1) A multinucleate cell or structure formed by the
cytoplasmic fusion, without nuclear fusion, of a number of
individual mononucleate protoplasts or cells (see e.g. GIANT
CELLS). (2) Syn. COENOCYTE.
syndrome (med., vet.) A group of symptoms and/or signs which,
taken together, characterize or are indicative of a distinct disease
or abnormality.
Synechococcus A genus of unicellular CYANOBACTERIA (section
I) in which the cells are often more or less rod-shaped, occur
singly, contain thylakoids, and lack a sheath; division occurs
by equal binary fission in one plane. This genus [see JGM
(1979) 111 161] includes organisms with a wide range of types
of morphology, physiology, GC% (3971), etc, and proposals
have been made to subdivide the genus into four genera [Ann.
Mic. (1983) 134 B 2136]: Cyanobacterium (GC%: 3941,
cells 1.72.3 m wide); Cyanobium (GC%: 6671, cells ca.
0.81.4 m wide); Cyanothece (GC%: ca. 42, cells ca. 46 m
wide); Synechococcus (GC%: 4756, cells 12(3.5) m wide).
These organisms occur in a wide range of habitats: e.g., as plankton
in the open ocean [Nature (1979) 277 293294], in hypersaline
environments such as salt evaporation ponds (e.g. Cyanothece
(Aphanothece) halophytica), and in hot springs e.g. S. lividus
can grow at temperatures up to ca. 70 C.
Certain strains of Synechococcus (sensu lato) exhibit a
swimming (not gliding) motility even though the organisms
lack flagella; swimming speeds are 525 m/sec, and the type
of swimming is influenced by cell morphology: coccoid cells
carry out looping and spiral movements, while rods move in
relatively straight paths [Science (1985) 230 7476]. Flagellumless, calcium-dependent motility (of unknown mechanism) has
been reported in strains of Synechococcus [JB (1997) 179
25242528].
Circadian regulation of the gene psbAI (which encodes a component of photosystem II) has been studied in Synechococcus
[TIM (1998) 6 407410].
Synechocystis A genus of unicellular CYANOBACTERIA (section
I) in which the cells are coccoid and divide by equal binary
non-electrogenic as e.g. when an anion is transported in symport with a cation. (cf. ANTIPORT, UNIPORT; see also ION TRANSPORT.)
synanamorph (mycol.) One of two or more ANAMORPHS of a
given TELEOMORPH.
synapsis The pairing of homologous chromosomes during MEIOSIS, or the juxtaposition of homologous regions of DNA prior to
general RECOMBINATION e.g. in prokaryotes, or the juxtaposition
of appropriate sequences prior to SITE-SPECIFIC RECOMBINATION.
synaptobrevin See TETANOSPASMIN.
synaptonemal complex A structure, visible by electron microscopy, which lies between homologous chromosomes in the
early stages of MEIOSIS; it consists of three parallel electron-dense
strands (a central element sandwiched between two lateral
elements) the whole being aligned with the long axis of the
homologous pair of chromosomes, and interposed between them.
One or more rounded or elongated structures (recombination
nodules) may be embedded within, or may bridge, the synaptonemal complex; these nodules may be involved e.g. in the
initiation of recombination since their number and distribution
appear to coincide with those of the chiasmata.
syncaryon Syn. SYNKARYON.
Syncephalastraceae See MUCORALES.
Syncephalastrum See MUCORALES.
synchronous culture A form of CULTURE (sense 2) in which all
the cells pass through the same stage of the CELL CYCLE at the
same time. Synchronous culture is used e.g. to study particular
biochemical events at specific stage(s) of the cell cycle.
Synchrony may be achieved in various ways. For example,
synchronous cultures of certain algae can be obtained by
the use of controlled cycles of light and dark. Synchrony in
bacterial cultures may be achieved by subjecting the cells, for
a given period of time, to an inhibitor of protein synthesis (e.g.
chloramphenicol). Yeast cultures have been made synchronous
by the use of EDTA or the IONOPHORE A23187 [JGM (1979)
114 391400]. Synchronous cultures of Tetrahymena pyriformis
have been obtained by heat shock: the brief exposure of a nonsynchronous culture to an elevated temperature (e.g. 40 C). All
of these methods, however, tend to perturb normal metabolic
activity so that they may be unsuitable for use in studies on cellcycle-linked physiology. A method which avoids this problem
can be used for endospore-forming bacteria; in this method a
population of endospores is induced to germinate at a given time
so that the resulting vegetative cells at least initially behave
synchronously.
A more generally applicable method of obtaining synchronous
cultures is termed selection synchrony; in this method, cells at
a given stage of the cell cycle are separated out from a nonsynchronous culture by purely physical means. In one selection
method (used e.g. to obtain synchronous bacterial cultures)
advantage is taken of the fact that the mass:volume ratio of the
cell varies during the cell cycle; a non-synchronous, log-phase
culture is subjected to density gradient CENTRIFUGATION so that
the fraction of maximum density (consisting of cells about to
divide, and new daughter cells) can be separated from the leastdense fraction which consists of a population of cells at a
particular stage of the cell cycle. [Selection synchrony method
for bacterial cultures: Book ref. 2, pp. 166168.] A selection
method has also been used e.g. with cultures of Dictyostelium
discoideum [JGM (1982) 128 24492452].
Synchronization of mammalian cells (e.g. in tissue cultures)
may be achieved e.g. by the double thymidine blockade. A
non-synchronous culture is exposed to a high concentration of
755
Synercid
of biosynthetic pathways. AUXOTROPHS which have blocks at
different points in the same pathway may exhibit a syntrophic
relationship: a substrate of a particular blocked reaction tends to
accumulate and diffuse into the surrounding medium, supporting
the growth of any auxotrophs blocked at earlier stages in the
common pathway.
Syntrophobacter
A genus of Gram-negative, anaerobic, nonmotile bacteria which oxidize propionate to acetate, CO2 and
H2 ; growth occurs only in the presence of H2 -scavenging
systems e.g. in co-culture with Desulfovibrio in the presence
of sulphate. [Genus proposed in AEM (1980) 40 626632.] (cf.
SYNTROPHOMONAS.)
Syntrophomonas A genus of Gram-negative, anaerobic bacteria
which can use only protons as electron acceptors in the oxidation
of short-chain fatty acids (e.g. butyrate) to acetate (or to a
mixture of acetate and propionate); the organisms can grow
only in the presence of H2 -scavenging systems e.g. in coculture with methanogens (see ANAEROBIC DIGESTION). Cells:
round-ended, curved or helical rods with 28 flagella arising
from the concave side of the cell. (cf. SYNTROPHOBACTER.)
Syntrophus A proposed genus of Gram-negative anaerobic bacteria. S. buswellii, the type species, was isolated from anaerobic digester sludge. Cells: round-ended rods with monotrichous
polar flagella in the early stages of growth. Benzoate is metabolized with the formation of acetate, CO2 and H2 (or formate).
Growth is inhibited by H2 and requires the presence of appropriate hydrogenotrophic bacteria. [IJSB (1984) 34 216217.]
syntype (cotype) Each of several specimens none having been
designated a HOLOTYPE on which an author has based a
published description of a new taxon.
Synura
A genus of colonial CHRYSOPHYTES. Each elongatepyriform cell has two flagella of similar length. The cells are
compactly arranged flagellate (anterior) ends outwards in a
globular, motile colony (100400 m diam.). Intricate siliceous
spicules occur at the anterior end of each cell. Species occur
in freshwater lakes and reservoirs with hard water, sometimes
forming blooms; S. petersenii has been implicated as a cause of
obnoxious fishy taste and odour in lake waters [CJB (1985) 63
14821493].
syphilis A chronic human disease caused by Treponema pallidum. Infection generally occurs by direct contact with lesions
of primary or secondary syphilis (see T. pallidum under TREPONEMA; see also VENEREAL DISEASE); T. pallidum can apparently
penetrate undamaged mucous membranes, and is rapidly disseminated through the body via the blood and lymphatic systems.
Primary syphilis. The first clinical manifestation is the chancre: a relatively painless, indurated lesion which develops at
the infection site ca. 1090 days after infection; in women the
chancre may develop on the cervix and may thus be undetected.
The chancre heals, without treatment, after ca. 1040 days. Secondary syphilis begins one to several months after the disappearance of the chancre, and involves e.g. a rash of cutaneous lesions
(which may be papular, macular, wart-like etc), thin white sores
on the mucous membranes (mucous patches), loss of hair, lymphadenopathy, and mild general symptoms (slight fever, malaise
etc). GLOMERULONEPHRITIS may occur. Latent syphilis occurs
between the (spontaneous) disappearance of secondary symptoms and the development of late syphilis. The latent infection
may persist for 140 years or more; there is no clinical evidence of infection (although symptoms of secondary syphilis
may recur), but serological tests may be positive. Late syphilis
(tertiary syphilis) may involve any tissue or organ e.g., skin,
bones, eyes (often leading to blindness), CNS (leading e.g. to
syzygy
disease. PCR amplified regions within tpn47 (a gene encoding the major treponemal membrane lipoprotein), fragments
being analysed by (i) gel ELECTROPHORESIS and (ii) Southern
hybridization (see SOUTHERN BLOT) [Lancet (2002) 360 388
389].
syringomycin A peptide-containing phytotoxin, produced by
Pseudomonas syringae pv. syringae, which causes a rapid,
detergent-like lysis of plant and fungal cytoplasmic membranes.
(cf. SYRINGOTOXIN.) [Regulation of syringomycin production:
JAB (1985) 58 167174.]
syringotoxin A phytotoxin produced by citrus-infecting strains
of Pseudomonas syringae [PPP (1981) 18 4150]. (cf. SYRINGOMYCIN.)
systematics (1) Syn. TAXONOMY. (2) The range of studies (theoretical and practical) involved in the classification of organisms.
syst`eme secant (ciliate protozool.) A line, marked by the
absence of kinetosomes, which delimits adjacent groups or fields
of kineties. Examples include e.g. the preoral suture (which
typically runs along the ventral surface between the oral region
and the anterior pole) and the postoral suture (which typically
runs, ventrally, between the oral region and the posterior
pole).
systemic (1) (med., vet.) Involving the whole body. (2) (plant
pathol.) Refers to a chemical agent (e.g. an ANTIFUNGAL AGENT)
which penetrates and is translocated within the tissues of a plant.
systole See CONTRACTILE VACUOLE.
syzygy In certain protozoa; a stage of sexual reproduction in
which gametocytes become physically joined without losing
their identity as separate cells. A pair of cells in syzygy usually
encysts and gives rise to male and female gametes.
757
Dictionary of Microbiology and Molecular Biology, Third Edition Paul Singleton and Diana Sainsbury
2006 John Wiley & Sons Ltd. ISBN: 0-470-03545-5
T
collar bearing six whiskers to a tail (ca. 100 22 nm)
consisting of two coaxial tubes (an inner core and an outer
contractile sheath). The distal end of the tail terminates in
a hexagonal base-plate consisting of a central hub or core
surrounded by six wedges. In T4, the hub contains at least 8
proteins including a thymidylate synthase (gptd), a glutamyl
carboxypeptidase (gp28), an ATP-requiring folyl polyglutamyl
synthetase (gp29), and a lysozyme (gp5) which is apparently
able to induce LYSIS FROM WITHOUT as well as lysis from within
[JV (1985) 54 460466]; the hub also contains dihydropteroyl
(dihydrofolyl) hexaglutamate. The wedges each contain at least
six proteins, including a dihydrofolate reductase (gpfrd). Each
corner of the base-plate bears a long jointed tail fibre (ca.
150 34 nm) and a short tail fibre (ca. 35 34 nm) the
latter containing zinc.
The phage genome consists of a linear, circularly permuted,
terminally redundant dsDNA molecule ca. 170 kb long (including the terminal redundancy of ca. 2.3%). The DNA contains
hydroxymethylcytosine (HMC) instead of cytosine, and may also
be modified by glucosylation of HMC residues and (in T2 and
T4, but not in T6) N6 -methylation of a small proportion of the
adenine residues.
See BACTERIOPHAGE T4 for infection cycle.
T helper cell (Th ; TH ) See T LYMPHOCYTE.
T-independent antigen THYMUS-INDEPENDENT ANTIGEN.
T lymphocyte (T cell) A type of LYMPHOCYTE involved in e.g.
ANTIBODY FORMATION, CELL-MEDIATED CYTOTOXICITY, INFLAMMATION and DELAYED HYPERSENSITIVITY. There are various types
(subsets) of T cell, each subset being distinguishable by function and/or cell-surface antigens. Like B LYMPHOCYTES, T cells
develop from haemopoietic stem cells (in the bone marrow)
via the lymphoid pathway of development. The (morphologically distinguishable) large granular lymphocytes known as NK
CELLS also develop from T cell precursors; NK cells are thus
related to, but distinct from, T cells. (Other leukocytes, including macrophages and PMNs, develop from haemopoietic stem
cells via the myeloid pathway.)
An antigen-specific T CELL RECEPTOR enables each T cell to
respond to a unique antigen (T cells in the same clone responding
to the same antigen). Unlike B cells (which bind soluble, i.e. free
or isolated, antigen), T cells react to specific antigen only when
it appears in suitable form on the surface of another cell; for
example, during the process of ANTIBODY FORMATION, a T cell of
a particular subset interacts with antigen presented in association
with an MHC class II molecule on the surface of a B cell.
Cytotoxic T cells (see later) interact with ligands on their target
cells; cytotoxic cells have the important function of killing host
cells that are infected with e.g. viruses or intracellular bacteria.
In general, when a T cell interacts with its specific antigen the T
cell is induced to proliferate (i.e. multiply), thus forming a clone
(or a larger clone) of cells reactive to that specific antigen; such
proliferation of a T cell of given antigenic specificity is called
clonal expansion.
Although T cells respond to antigens only when the latter
are cell-associated, they can respond to other isolated (soluble)
molecules such as CYTOKINES.
Unlike B cells, most or all T cells undergo their process of
maturation in the thymus gland. (The mouse is reported to have a
tactic response
negatives), can recognize non-peptide antigens; for example
mycobacterial cell components, including mycolic acids, can be
recognized by the ab-type cells.
T-lysin See FURUNCULOSIS (sense 1).
T number See ICOSAHEDRAL SYMMETRY.
T odd phages Bacteriophages T1 and T5 (STYLOVIRIDAE) and T3
and T7 (PODOVIRIDAE).
T protein (T antigen) (in streptococci) A cell-surface protein
found in certain group A streptococci. T proteins are not
associated with virulence, but are highly antigenic and may be
used in typing of group A streptococci. Particular T-antigenic
types are usually associated with particular M-antigenic types
(see M PROTEIN sense 1). (cf. R PROTEIN.)
T-strain mycoplasmas Earlier name for members of the genus
UREAPLASMA.
T-strand See CONJUGATION (1b)(i).
T1 side-chains See O ANTIGENS.
T-2 toxin A TRICHOTHECENE mycotoxin.
T2H test (TCH test) A test used in the identification of strains
of Mycobacterium. Essentially, the test determines the ability
of a given strain to grow (positive result) on a medium (e.g.
LowensteinJensen medium) containing thiophene-2-carboxylic
acid hydrazide (T2H, TCH) often at 10 g/ml, a concentration
inhibitory to M. bovis but not to most strains of M. tuberculosis;
those strains of M. tuberculosis which are inhibited by 10 g/ml
T2H may be able to grow on media containing 15 g/ml (concentrations still inhibitory to M. bovis) [Book ref. 53, p. 1710].
T7 phage group A genus of phages of the PODOVIRIDAE. Type
species: BACTERIOPHAGE T7; other members: e.g., bacteriophages
T3, W31, fI and fII.
T90 The time required for 90% mortality to occur in a population
of microorganisms exposed to a given hostile regime.
TAB An INACTIVATED VACCINE containing the cells of Salmonella
typhi and S. paratyphi A and B.
Tabellaria See DIATOMS.
TABT TAB vaccine incorporating tetanus toxoid.
tabtoxin A b-lactam-containing dipeptide toxin produced by e.g.
Pseudomonas syringae pv. tabaci. In the tobacco plant, tabtoxin
is enzymically hydrolysed to tabtoxinine-b-lactam which inhibits
glutamine synthetase; the consequent accumulation of ammonia
appears to be an important factor in the pathogenesis of WILDFIRE
DISEASE. [APRpath. (1984) 22 218221; susceptibility of bacterial glutamine sythetase to tabtoxinine-b-lactam: JGM (1985)
131 10611067; contribution of tabtoxin to the pathogenicity
of Pseudomonas syringae pv. tabaci : PPP (1984) 25 5569.]
Tabtoxin-producing strains of P. syringae can be detected
rapidly by PCR-based methodology [LAM (2001) 32 166170].
Tac antigen A T lymphocyte surface antigen associated with the
receptor for INTERLEUKIN-2.
tac promotor A hybrid PROMOTER constructed in vitro by fusion
between elements of the lac and trp promoters of Escherichia
coli (see LAC OPERON and TRP OPERON). The tacI promoter
contains the Pribnow box from the lac promoter and the 35
sequence from the trp promoter; tacII contains the trp 35
sequence but its Pribnow box is a hybrid between those of the
trp and lac promoters. The tac promoters are stronger than either
parent promoter; they can be repressed by the lac repressor and
induced by IPTG.
Tacaribe virus See ARENAVIRIDAE.
tache noir See BOUTONNEUSE.
tachyzoite Syn. ENDOZOITE.
TACTAAC box See SPLIT GENE (a).
tactic response Syn. TAXIS.
tactophily
Tanapox virus A virus of the POXVIRIDAE which can infect
humans, causing an acute, febrile illness with localized, pocklike skin lesions; the illness has occurred in epidemics among
people in the region of the Tana River, Kenya. Tanapox virus
can also infect monkeys. It does not grow in the CAM but can be
cultivated in monkey kidney cell cultures. In serological tests the
Tanapox virus shows partial cross-reactivity with YABA MONKEY
TUMOUR POXVIRUS.
TANDEM See QUINOXALINE ANTIBIOTICS.
tane koji See KOJI.
tanned cells See BOYDEN PROCEDURE.
tanned ox haemagglutination See FIMBRIAE.
tannic acid (1) Penta-(m-digalloyl)-glucose, a hydrolysable tannin. (2) Any hydrolysable tannin (see TANNINS).
tannins A heterogeneous group of complex polyhydroxybenzoic
acid derivatives which occur e.g. in plants and in brown algae
(see PHAEOPHYTA). Hydrolysable tannins consist of a sugar
(often glucose) partially or wholly esterified with e.g. gallic
acid (3,4,5-trihydroxybenzoic acid), digallic acid (a DEPSIDE),
or ellagic acid; hydrolysis yields the component sugar and
acids. Condensed (non-hydrolysable) tannins are believed to be
oligomers of flavanoid compounds; they tend to polymerize (e.g.
under acid conditions) to form insoluble reddish compounds
(phlobaphenes).
Tannins can precipitate and inactivate proteins by forming
cross-links (a property exploited e.g. in leather tanning and in
the BOYDEN PROCEDURE). In plants, tannins occur mainly in bark
and woody tissues but also in certain leaves (e.g. tea-leaves);
they may occur in vacuoles, in cell walls, or in specialized cells.
They are also formed in damaged plant tissues as a result of
the oxidation (in the presence of air) of phenolic compounds in
the cell vacuoles by polyphenoloxidases normally sequestered in
lysosomes. Tannins are believed to play a role in the resistance
of plants to disease: e.g., by inhibiting enzymes (such as PECTIC
ENZYMES) produced by invading pathogens, and by binding to
and reducing the availability of proteins in the damaged plant
tissue.
A comparison of two species of rumen bacteria, Streptococcus
bovis and S. gallolyticus (= S. caprinus), found that the latter
species can adapt to higher levels of tannins e.g. by upregulating
the enzyme gallate decarboxylase and forming an extracellular
polysaccharide matrix [Microbiology (2001) 147 10251033].
tap gene See CHEMOTAXIS (Escherichia coli ).
Taphrina
A genus of dimorphic fungi (order TAPHRINALES)
which include species parasitic e.g. on various trees including
alder (Alnus); birch (Betula); cherry, peach and plum (Prunus);
and oak (Quercus). Taphrina spp form an intercellular or
subcuticular septate mycelium; some species form haustoria.
Asci (see ASCUS) may develop as a subcuticular, erumpent
layer, each ascus (containing ovoid or spheroidal ascospores)
developing from a cell produced by hyphal fragmentation. In
culture, Taphrina spp may grow only in a budding, yeast-like
form.
T. deformans can cause e.g. WITCHES BROOM and peach (and
almond) leaf curl. In leaf curl, the young leaves become distorted
and yellowish with reddish patches, and a white or silvery film
develops on their upper surfaces; the leaves later become brown
and drop prematurely. Young shoots, flowers and fruit may also
become distorted.
Taphrinales An order of plant-parasitic fungi of the subdivision
ASCOMYCOTINA. Ascocarps are not formed; the asci develop,
directly or indirectly, from the hyphae, or from individual cells
formed by the fragmentation of hyphae. Genera: e.g. TAPHRINA.
taxon
numbers of target molecules), permits estimates to be made from
samples in which the initial target numbers are unknown.
Threshold cycles in PCR can also be determined with MOLECULAR BEACON PROBES (q.v.); fluorescence levels from these probes
are recorded, cycle-by-cycle, at the primer annealing stage (when
the amplicon-bound probes are fluorescent).
TaqMan probes have been used e.g. for the quantitative
estimation of Borrelia burgdorferi in specimens of tissue [JCM
(1999) 37 19581963].
tar gene See CHEMOTAXIS (a).
tar spot See RHYTISMA.
tartar emetic See ANTIMONY.
tartronic semialdehyde pathway See TCA CYCLE [and Appendix II(b)] and PHOTORESPIRATION.
Tat See PROTEIN SECRETION (end of type II systems).
TATA box See PROMOTER.
TATA box-binding protein See PROMOTER.
Tatlockia See LEGIONELLACEAE.
Tatumella A genus of bacteria of the ENTEROBACTERIACEAE, isolated from human clinical (usually respiratory tract) specimens.
Non-motile at 36 C; many strains are motile at 25 C [JCM
(1981) 14 7988].
t (superhelix winding number) See DNA.
tau protein See MICROTUBULE-ASSOCIATED PROTEINS.
Tauber trap A simple instrument used for sampling airborne
particles. (See also AIR.) It consists of a cylindrical vessel with
an aerodynamically shaped lid containing a central hole.
Taumelkrankheit In fish: a loss of muscular coordination leading
to a spiral swimming motion; it may be a (uncommon) symptom
of ICHTHYOPHONOSIS or of thiamine deficiency.
taurine An aminosulphonic acid (NH2 CH2 CH2 SO3 H) derived
from cysteine; it occurs e.g. conjugated with BILE ACIDS.
taurocholic acids See BILE ACIDS.
taurolin A wide-spectrum FORMALDEHYDE-releasing antimicrobial agent which has been used e.g. for the treatment of peritonitis. [Review: JAB (1980) 48 8996.]
taxa Plural of TAXON.
taxis A locomotive response to an external stimulus, exhibited by
certain (motile) cells or organisms, in which the direction or
net change in direction of locomotion is related to the direction
or orientation of the stimulus. (cf. KINESIS; TROPISM.) In general, a
tactic response is triggered only when the level of the stimulus is
above a minimum (threshold) value; however, extreme levels of
stimulation may promote tactic responses different from those
produced by moderate stimulation (see e.g. PHOTOTAXIS). (See
also ADAPTATION.)
In bacteria, some taxes depend on changes in the cells
proton motive force (see e.g. AEROTAXIS and PHOTOTAXIS; cf.
CHEMOTAXIS). [Pmf-dependent taxis: ARM (1983) 37 551573.]
See also e.g. ELASTICOTAXIS; GALVANOTAXIS; GEOTAXIS; MAGNETOTACTIC BACTERIA; RHEOTAXIS; THIGMOTAXIS.
taxol A complex substance of plant origin (obtained from Taxus
brevifolia) which has antitumour activity, and which can e.g.
inhibit the growth of HeLa cells at a concentration of 0.25 M.
Taxol apparently enables the assembly of MICROTUBULES to occur
with very low concentrations of tubulin (ca. 0.01 mg/ml in
vitro) i.e., it decreases the value of the critical concentration
of tubulin thereby promoting microtubule assembly; it also
stabilizes MTs and (hence) prevents a cell from disassembling
its MTs preparatory to the formation of a mitotic spindle. Taxol
permits in vitro assembly of MTs in the absence of GTP.
taxometrics Syn. NUMERICAL TAXONOMY.
taxon (pl . taxa) In a given system of biological classification:
any category, consisting of one or more kinds of organism,
taxonomy
regarded as having an identity distinct from that of any other
category in that system; a taxon may be a group of strains,
species, genera, etc.
taxonomy The science of biological classification, i.e. the grouping of organisms according to their natural affinities. (cf. SYSTEMATICS.) A classified arrangement of organisms permits a logical
and informative system of naming (see NOMENCLATURE) and can
also be useful e.g. for identifying newly isolated organisms.
Ideally, biological classification should reflect the natural
(evolutionary) relationships between organisms (i.e. PHYLOGENETIC CLASSIFICATION; cf. PHENETIC CLASSIFICATION). Such a
phyletic approach has been used traditionally in taxonomic
schemes for higher animals and plants (in which evolutionary
relationships can be deduced from structural and other features).
However, among microorganisms, the prokaryotes have (until
recently) presented particular difficulties for taxonomists, and
earlier forms of classification tended to suffer from artificiality
and subjectivity; attempts to introduce a more rational basis for
the taxonomy of these organisms lead to increased interest in e.g
NUMERICAL TAXONOMY. (An objective approach was also sought
in areas such as enzymological analysis [e.g. CRM (1982) 9
227252], protein structure (MICROCOMPLEMENT FIXATION), RIBOSOME structure, and the sequence of loci in the genome [IJSB
(1985) 35 217220].)
The modern approach to prokaryotic taxonomy began with
molecular studies in which organisms are compared and classified according to the sequences of nucleotides in their nucleic
acids (see e.g. RRNA OLIGONUCLEOTIDE CATALOGUING and DNA
HOMOLOGY). Thus, the concept of a SPECIES (q.v.) may be considered in terms of the similarity (%) between chromosomal DNA
from different strains; moreover, different species in a given
genus commonly exhibit a certain minimum level of difference
in their 16S rRNA sequences. However, reliance on 16S rRNA
sequences as a guide to species identity has been questioned
[IJSB (1992) 42 166170]. (16S rRNA is widely used for the
phyletic classification of prokaryotes for two main reasons. First,
it occurs in all prokaryotes. Second, it contains highly conserved
(i.e. stable) sequences as well as more variable sequences; the
highly conserved sequences are considered to be appropriate for
classification at the higher end of the taxonomic spectrum e.g.
kingdom, domain while variable sequences are deemed to be
useful for lower-rank taxa.) 16S rRNA oligonucleotide cataloguing initially revealed two kingdoms Archaebacteria and
Eubacteria each later elevated to domain status (Archaea and
Bacteria, respectively).
There is also a consensus form of taxonomy polyphasic
taxonomy in which the aim is to base classification on the
maximum amount of information available, including both
phenotypic and molecular data [polyphasic taxonomy: MR
(1996) 60 407438].
A taxonomic hierarchy is a classificatory system in which a
single, all-inclusive category (e.g. bacteria or fungi) is progressively divided into smaller and less-inclusive categories, all
the organisms in a given category conforming to the same criteria
(i.e. all having, or lacking, certain feature(s)). A taxonomic hierarchy may have the following principal ranks (listed in descending order of inclusiveness): division (in botanical schemes) or
phylum (in zoological schemes); class; order; family; genus;
SPECIES; one or more species constitute a genus, one or more
genera constitute a family, and so on. There are also intermediate ranks: see e.g. the table in the entry NOMENCLATURE. (See
also FORM GENUS and SACCARDOAN SYSTEM.) A species can be
subdivided into STRAINS which are distinguishable by TYPING
procedures. (See also FORMA SPECIALIS; SEROTYPE; VARIETY.)
tecnazene
conditions are such that some of the enzymes are necessary for
biosynthesis, the levels of those enzymes are increased despite
anaerobiosis; under such conditions 2-oxoglutarate dehydrogenase (= a-ketoglutarate dehydrogenase) remains repressed and
the pathway ceases to be cyclic, functioning in biosynthesis
as two linear pathways: an oxidative pathway from citrate to
2-oxoglutarate, and a reductive pathway from OAA to succinylCoA. 2-Oxoglutarate dehydrogenase is also repressed by anaerobiosis in many other facultatively anaerobic organisms. The
TCA cycle is inherently incomplete in some bacteria: e.g. in
cyanobacteria, in Gluconobacter, and in some members of the
Methylococcaceae; in at least some cyanobacteria succinyl-CoA
is formed via the glyoxylate cycle rather than via the reductive pathway from OAA. (See also GLUTAMIC ACID.) A complete
cycle is apparently involved in the oxidation of acetate by sulphate in the obligately anaerobic sulphate-reducing bacterium
Desulfobacter postgatei (see DESULFOBACTER), although some
of the enzymes involved are unusual in certain respects: e.g.,
malate and possibly succinate dehydrogenases appear to use
quinones instead of pyridine nucleotides as coenzymes, and 2oxoglutarate dehydrogenase is specific for a ferredoxin instead of
NAD+ as electron acceptor. In D. postgatei, pyruvate (and hence
OAA) can be synthesized from acetyl-CoA by direct reductive
carboxylation catalysed by a ferredoxin-dependent pyruvate synthase.
[Bacterial TCA cycle enzymes (particularly citrate synthase
and succinate thiokinase): AMP (1981) 22 185244.]
(See also REDUCTIVE TRICARBOXYLIC ACID CYCLE.)
TCBS agar Thiosulphatecitratebile salts agar: a medium
containing peptone, sucrose, thiosulphate, citrate, cholate, oxgall,
ferric citrate, NaCl, thymol blue, and bromthymol blue [recipe:
Book ref. 46, p. 1276]. It is used for the isolation of Vibrio spp,
especially V. cholerae; sucrose-fermenting strains form yellow
colonies. The medium is strongly inhibitory for most faecal
enterobacteria, pseudomonads, and Gram-positive bacteria.
TCC See CARBANILIDES.
TCCR (cytokine receptor) See CYTOKINES.
TCD50 An alternative expression for TCID50 (q.v.).
tcdA, tcdB, tcdE genes See LYSIS PROTEIN (sense 3).
TCGF See INTERLEUKIN-2.
TCH test Syn. T2H TEST.
TCID50 (TCD50 ) Tissue culture infective dose (50%): that dose
of a viral suspension which, when used to inoculate each of a
number of TISSUE CULTURES, causes observable effects in 50% of
those cultures. (See also END-POINT DILUTION ASSAY.)
TCNB See TECNAZENE.
TCP Toxin co-regulated pili: see CHOLERA, BACTERIOPHAGE CTX8
and PATHOGENICITY ISLAND.
TCR See T CELL RECEPTOR.
tD See THERMAL DEATH TIME.
TD antigen THYMUS-DEPENDENT ANTIGEN.
td gene (in bacteriophage T4) See SPLIT GENE.
TDH See FOOD POISONING (Vibrio).
tDNA DNA which encodes tRNA.
T-DNA See CROWN GALL.
tea diseases Diseases of the tea plant, Camellia sinensis (=
Thea sinensis), include e.g. BLISTER BLIGHT and RED RUST.
teart See SCOURS.
teat (microbiol.) A rubber bulb used e.g. for operating a pipette.
tecnazene (TCNB) An agricultural antifungal agent (2,3,5,6tetrachloronitrobenzene) used e.g. (as a dust) for the control
of dry rot (Fusarium coeruleum) of stored potatoes; it also
inhibits the sprouting of stored potatoes. TCNB is also used (as
763
Tectibacter
a smoke) in glasshouses for the control of Botrytis infections.
(cf. QUINTOZENE.)
Tectibacter A genus of Gram-negative bacteria which occur as
endosymbionts in the cytoplasm of strains of Paramecium aurelia. Cells: peritrichously flagellated straight rods, ca. 0.40.7
1.02.0 m. No strains appear to be toxic to protozoa. Type
species: T. vulgaris (earlier name: delta particles).
[Book ref. 22, p. 811.]
Tectiviridae (PRD1 phage group) A family of lipid-containing,
icosahedral BACTERIOPHAGES (diam. (53-)65(-80) nm) which
contain linear dsDNA (MWt ca. 107 ). One genus: Tectivirus;
type species: phage PRD1. Host range for the family includes
Gram-negative and Gram-positive bacteria. Phage progeny are
released by cell lysis. Plaques: clear or turbid, minute to large.
The virion contains a dense core, probably solely of DNA,
surrounded by a lipid bilayer the whole being enclosed by
the icosahedral protein shell; single spikes (ca. 20 nm long)
are sometimes seen on the vertices. Some virions have a tail
(length variable) which appears when DNA is ejected or virions
are damaged and which may be part of a mechanism for DNA
ejection. Virions are sensitive to organic solvents and detergents.
Phages PRD1, PR3, PR4, PR772 (probably = PR4), PR5 and
L17 are closely related and are specific for Gram-negative
bacteria (e.g. Escherichia coli, Salmonella typhimurium, Pseudomonas aeruginosa) which harbour IncN, IncP1 or IncW plasmids. The site of phage adsorption is controversial: phage may
adsorb to pili (which may then retract) or directly to the cell
surface.
Other tectiviruses attack Bacillus spp. Phages AP50 (host:
some strains of B. anthracis) and Bam35 (hosts: B. cereus,
B. megaterium, B. thuringiensis) are very similar and are both
highly sensitive to heat. Phage fNS11 is acidophilic and
thermophilic (as is its host, B. acidocaldarius). fNS11 is stable
at pH 25 but is rapidly inactivated at pH above 6; it
contains the unusual !-cyclohexyl fatty acids characteristic of
B. acidocaldarius cell membranes.
Tectivirus See TECTIVIRIDAE.
tectum (protozool.) See COCHLIOPODIUM.
teeth (diseases of) See DENTAL CARIES and PERIODONTITIS.
Teflon filter See FILTRATION.
Tego compounds A range of antimicrobial ampholytic surfactants used e.g. as antiseptics and disinfectants; an example
is Tego 103S (dodecyl-di(aminoethyl)-glycine hydrochloride).
[Book ref. 65, pp. 335345.]
tegulicolous Growing on tiles.
tegument See HERPESVIRIDAE.
teichoic acids (TAs) Polymers which typically consist mainly
of glycerol phosphate or ribitol phosphate (or rarely mannitol
phosphate) substituted more or less extensively with amino acids
and/or sugars; they occur in the cell envelope in most Grampositive bacteria. (TAs are very rare in Gram-negative bacteria,
but have been found in strains of Butyrivibrio and of Escherichia
coli see below.)
Glycerol teichoic acids (GTAs) occur in the CYTOPLASMIC MEMBRANE, in the periplasmic region, and/or in the CELL WALL; they
are commonly composed of glycerol residues linked 1 3 by
phosphodiester bridges and substituted with e.g. D-alanine, Nacetylglucosamine (GlcNAc), glucose, KOJIBIOSE, etc. (See also
C SUBSTANCE.) In some GTAs a sugar forms an integral part of
the polymer backbone. (The K2 capsular antigen of E. coli contains alternating galactofuranosylglycerol phosphate and galactopyranosylglycerol phosphate residues [Biochem. (1982) 21
12791284].)
terbutryne
telotroch The motile (ciliated) immature stage of a sedentary
peritrich. (See also TROCHAL BAND.)
TEM See ELECTRON MICROSCOPY (a).
TEM-1 b-lactamases See b-LACTAMASES.
TEM-2 b-lactamases See b-LACTAMASES.
tempeh (tempe kedelee) A food, originally from Indonesia, consisting of soybeans fermented and bound into a cake by
mycelium of Rhizopus spp (e.g. R. oligosporus); a strain of
Klebsiella pneumoniae is also present and contributes vitamin
B12 to the product [Book ref. 6, pp. 414416]. Soybeans are
soaked, dehulled, boiled, surface-dried, and mixed with an inoculum of Rhizopus sp; the beans are then packed tightly into a
container and incubated until they are coated and bound by an
abundant white mycelium (e.g. 32 C for ca. 20 hours). Bongkrek
(tempe bongkrek ) is a similar product made from coconut presscake or grits remaining after the extraction of coconut oil;
fermentation may be carried out by R. oligosporus or by Neurospora intermedia. (See also BONGKREKIC ACID; cf. ONCOM.)
[Tempe (recent data): Book ref. 228.]
temperate bacteriophage A BACTERIOPHAGE which can lysogenize its host cell (see LYSOGENY). (cf. VIRULENT BACTERIOPHAGE.)
temperature coefficient (q; Q) Of a given DISINFECTANT acting
on a single-species population of microorganisms: a coefficient
which indicates the factor by which the death rate increases
when the temperature rises by 1 C or, more commonly, 10 C,
in which case the temperature coefficient is designated q10 or
Q10 . The temperature coefficient for a given temperature range
(e.g. 1020 C) is not necessarily the same as that for other
ranges (e.g. 010 C; 2030 C).
temperature-sensitive mutant (ts mutant) A mutant (e.g. a CONDITIONAL LETHAL MUTANT) in which the mutated gene is functional at certain temperatures (permissive temperatures) but not
at others (non-permissive or restrictive temperatures); ts mutations are commonly MIS-SENSE MUTATIONS which alter an essential
protein such that it functions at the permissive temperature but
not at the restrictive (usually higher) temperature.
template strand (of DNA) See CODING STRAND.
temporal temperature gradient gel electrophoresis (TTGE)
See DGGE.
TEN TOXIC EPIDERMAL NECROLYSIS.
10 sequence See PROMOTER.
Tenericutes A proposed division of the PROCARYOTAE comprising
one class (MOLLICUTES).
tennecetin Syn. PIMARICIN.
tentoxin A cyclic tetrapeptide TOXIN produced by Alternaria spp;
it binds non-covalently to, and inhibits, (F0 F1 )-type PROTON
ATPASES, inducing chlorosis in various plants.
tequila See PULQUE.
teratogen Any agent which causes developmental abnormalities
in an embryo or fetus. (See also TORCH DISEASES; SYPHILIS.)
teratoma A neoplasm composed of more than one type of tissue.
terbinafine A synthetic allylamine antifungal agent which is used
clinically e.g. against dermatophyte infections.
The activity of terbinafine against Aspergillus spp has been
compared, in vitro, with the activities of itraconazole and
amphotericin B; compared with these two agents, terbinafine
had greater activity against A. flavus, A. terreus and A. niger
but it was less effective against A. fumigatus [AAC (2001) 45
18821885].
terbutryne An ALGICIDE and herbicide which is active against
a range of algae (e.g. species of Cladophora, Enteromorpha,
Rhizoclonium, Spirogyra) and against certain aquatic vascular
plants. It is useful for the control of algae and water-weeds in
static and slow-moving waters (lakes, canals, farm ponds, etc).
terconazole
terconazole See AZOLE ANTIFUNGAL AGENTS.
terete Circular in transverse section.
terminal deoxynucleotidyl transferase See TAILING.
terminal electron acceptor See e.g. RESPIRATION.
terminal protein (TP) See BACTERIOPHAGE f29.
terminal redundancy (mol. biol.) The presence of identical base
sequences at the two ends of a linear nucleic acid molecule.
In e.g. a terminally redundant dsDNA molecule, removal of
nucleotides from e.g. the 3 end of each strand results in the
formation of STICKY ENDS.
terminal transferase See TAILING.
termination codon See GENETIC CODE.
terminator See TRANSCRIPTION.
Termitaria A genus of fungi of the COELOMYCETES; T. snyderi
is parasitic on termites.
termitemicrobe associations Termites are social insects of the
Isoptera, found mainly in tropical regions; there are ca. 2000
species, many of which can feed on wood and can cause severe
economic damage in buildings etc. Many species depend on
symbiotic associations with microorganisms for the digestion of
cellulose and other components in their diet.
In lower termites (Hodotermitidae, Kalotermitidae, Mastotermitidae, Rhinotermitidae, Serritermitidae) the hindgut is
densely packed with microorganisms, including cellulolytic flagellate protozoa (e.g. TRICHONYMPHA) and various facultatively or
strictly anaerobic bacteria (e.g. strains of Bacillus, Bacteroides,
enterobacteria, spirochaetes (see SPIROCHAETALES), Staphylococcus and Streptococcus). The protozoa phagocytose particles of
cellulosic material ingested by the termite and ferment the cellulose to acetate, CO2 and H2 . Acetate is absorbed by the
termite and used as the major oxidizable energy source for termite metabolism. The H2 and CO2 are used by methanogens
and bacteria (possibly including Acetobacterium-like acetogens:
cf. ANAEROBIC DIGESTION). Other bacteria may generate acetate
and other volatile fatty acids from mono-, di- and oligosaccharides present in material ingested by the termite or released from
the protozoa. Thus, the protozoa are the main agents of cellulose degradation, while prokaryotes serve to remove H2 (which
would inhibit further cellulose degradation), maintain anaerobiosis, and possibly provide essential nutrients for the protozoa
which feed on them. Some of the bacteria are also important in
the nitrogen economy of the termite. The termites diet is often
low in nitrogen, and the gut bacteria may play an important role
by NITROGEN FIXATION and/or by recycling the nitrogen of uric
acid produced in the termite tissues; uric acid is passed into
the hindgut where it is used as an energy source by e.g. Bacteroides, Citrobacter, and Streptococcus spp, being fermented to
NH3 , CO2 and acetate. (cf. RUMEN.) The gut microflora is also
apparently involved in the degradation of other plant components (e.g. hemicelluloses, lignin), but the mechanisms are less
well understood. [Review: Book ref. 77, pp. 173203.]
In higher termites (Termitidae) the hindgut contains a large
population of bacteria [AEM (1985) 49 12261236] but no cellulolytic protozoa. Members of the subfamily Macrotermitinae
cultivate a fungus (Termitomyces sp) in fungus combs analogous to the FUNGUS GARDENS of the parasol ants; the termites
construct a comb from small fragments of plant tissue and termite faeces, and the surface of this comb becomes covered with a
sparse fungal mycelium which develops numerous white, spherical nodules (mycotetes
colonies are established, the inoculum of Termitomyces necessary for establishing a new fungus comb may be either carried (as
conidia) in the guts of the winged insects (e.g. in Macrotermes
bellicosus, Microtermes spp) or collected (as basidiospores) by
foraging workers (e.g. in Macrotermes subhyalinus, Ancistrotermes, Odontotermes).
(See also INSECTMICROBE ASSOCIATIONS.)
Termitomyces A genus of white-rot fungi (family Amanitaceae)
found only in certain termite nests (see TERMITEMICROBE
ASSOCIATIONS).
ternary combination In NOMENCLATURE: a designation which
consists of a binomial together with a subspecific epithet see
e.g. SUBSPECIES. (cf. TRINOMIAL.)
ternary fission An asexual reproductive process in which more
than two cells are formed from one cell (cf. BINARY FISSION);
ternary fission occurs e.g. in PELODICTYON.
terramycin See TETRACYCLINES.
Terrazole See ETRIDIAZOLE.
terregens factor See SIDEROPHORES.
terricolous Growing on soil, peat, sand etc.
tertian malaria See MALARIA.
Teschen disease A PIG DISEASE caused by a porcine ENTEROVIRUS;
it occurs e.g. in Central Europe and is named after the Teschen
(Cieszyn) district of (the former) Czechoslovakia. Symptoms
include fever followed by signs of encephalomyelitis: incoordination, tremors, convulsions and paralysis; the virus can be
isolated from the faeces of infected pigs. The mortality rate may
be 70% or higher, death occurring in 34 days. The disease
may be controlled by slaughter or by vaccination using a live,
attenuated vaccine. (cf. TALFAN DISEASE.)
tesla (T) A unit of magnetic flux density; 1 tesla = 10000 gauss.
TESPA See AAS.
test (protozool.) (1) A close-fitting protective shell which surrounds the cell e.g. in certain (testate) amoebae; the test may be
predominantly or entirely organic (as in e.g. ARCELLA) or may
incorporate inorganic materials such as sand grains (e.g. DIFFLUGIA), silica (e.g. EUGLYPHA), etc. (See also FORAMINIFERIDA.)
(2) Syn. LORICA.
test medium See MEDIUM.
Testacealobosia A subclass of testate amoebae (see ARCELLINIDA
and TRICHOSIDA). (cf. GYMNAMOEBIA.)
testate Possessing a TEST.
testosterone synthesis See STEROID BIOCONVERSIONS.
Tet protein See TETRACYCLINES.
tetA gene See TETRACYCLINES.
tetaine Syn. BACILYSIN.
tetanolysin A THIOL-ACTIVATED CYTOLYSIN produced by Clostridium tetani ; it is distinct from TETANOSPASMIN.
tetanospasmin (tetanus toxin) A plasmid-encoded neurotoxin,
produced by Clostridium tetani, which causes the symptoms of
TETANUS.
Tetanospasmin is a single polypeptide of 150 kDa. Activation involves proteolytic cleavage to form a di-chain structure
consisting of an H chain (100 kDa) and an L chain (50 kDa)
held together by a disulphide bond.
The activated toxin binds, via the H chain, to specific sites
on the cell membrane of a neurone at the nervemuscle
junction; receptor sites on the membrane may include (i)
polysialogangliosides and (ii) a specific protein.
Surface-bound toxin is internalized by uptake within a vesicle.
Toxin-containing vesicles are then translocated back along the
axon to interneurones in the spinal cord. According to one
model, release of the active component (the L chain) occurs after
766
tetra-O-di(biphytanyl) diglycerol
acidification of the vesicle has brought about a conformational
change in the H chain; the H chain may then insert into the
vesicles membrane and bring about the translocation of the
L chain from the vesicle to the cytoplasm of the neurone.
Reduction of the disulphide bond then releases the active toxin.
Normally, in the absence of toxin, contraction of a given
muscle stimulates the interneurones to release an inhibitory
neurotransmitter (?glycine) which prevents contraction of the
corresponding antagonist muscle. Neurotransmitter, present in
vesicles within the interneurone, is released into the (extracellular) synaptic cleft by a process in which the vesicles first dock
at specific sites on the (inner) surface of the cells membrane and
then fuse with the membrane (= exocytosis or neuroexocytosis);
this process is triggered by appropriate electrical stimulation and
the resulting intracellular rise in levels of Ca2+ .
During neuroexocytosis, docking and fusion of vesicles
involves specific interaction between molecules in the vesicle
membrane and others at the inner surface of the neurones membrane. These molecules include VAMP/synaptobrevin (VAMP =
vesicle-associated membrane protein), and (on the neurones
membrane) SNAP-25 and syntaxin.
Tetanospasmin acts as a zinc-endopeptidase which recognizes
and cleaves a specific molecule required for vesicle-docking in
neuroexocytosis, i.e. it prevents the docking of vesicles and
(thus) inhibits the release of neurotransmitter to the synaptic
cleft. Absence of the inhibitory neurotransmitter permits simultaneous contraction of both protagonist and antagonist muscles
in a given pair, thus giving rise to spastic (rigid) paralysis. The
target for tetanospasmin is apparently VAMP/synaptobrevin.
Tetanospasmin is also able to act peripherally, at the
nervemuscle junction, giving rise to a local, flaccid, paralysis.
[Mechanism of action of tetanus neurotoxin: Mol. Microbiol.
(1994) 13 18.]
tetanus (lockjaw) An acute disease, affecting man and animals,
caused by toxinogenic strains of Clostridium tetani. The disease develops when C. tetani contaminates wounds or other
lesions, especially those which have become anaerobic due e.g.
to necrosis or to infection with other bacteria; common sources
of C. tetani are faeces and soil. The incubation period may
be days or weeks; short incubation periods correlate with high
mortalities, and vice versa. Symptoms caused by TETANOSPASMIN may begin with stiffness or spasms of the jaw muscles,
typically followed by a generalized tetanus: movements or external stimuli (e.g. noise) trigger violent, painful, convulsive spasms
of the muscles in the trunk and limbs, and there is a characteristic contorted facial expression (risus sardonicus). Death
may result from asphyxia or exhaustion. Less common forms of
the disease include local tetanus (rigidity and increased muscle
tone in the vicinity of the infected wound) and cephalic tetanus
(in which certain cranial nerves becomes paralysed, usually following infection of a head lesion). Treatment may involve e.g.
administration of (preferably human) antitoxin, anticonvulsant
drugs, and/or neuromuscular blockade. Antitoxin may also be
used for short-term prophylaxis; longer-term (but still temporary) protection is achieved by vaccination with tetanus TOXOID.
(cf. DPT and TABT.)
tetanus toxin TETANOSPASMIN. (cf. TETANOLYSIN.)
tethering (of leukocytes) See INFLAMMATION.
tetracyclines A family of broad-spectrum ANTIBIOTICS whose
structure is based on the naphthacene skeleton (see figure); they
are produced by species of Streptomyces (e.g. S. aureofaciens,
S. rimosus) and/or made semi-synthetically.
The tetracyclines are used primarily as antibacterial (bacteriostatic) agents in the treatment of human and animal diseases
H3C
H3C
R2
OH
CH3
N
OH R
1
H
H
HO
OH
H
OH
CONH2
O
Tetragoniomyces
or both of the central microtubules of the axoneme. Biflagellate
isogametes are released from the colonies.
tetrasporal colony See TETRASPORA.
tetraspore A type of spore which develops in groups of four.
tetrasporic Of a coccidian oocyst: containing four sporocysts.
tetra-tetra dimers (in peptidoglycan) See PEPTIDOGLYCAN (figure
legend).
tetrathionate broth A medium containing peptone, bile salts,
sodium thiosulphate, and CaCO3 ; immediately before use, iodine
(in KI solution) is added (to convert thiosulphate, S2 O3 2 , to
tetrathionate, S4 O6 2 ), after which the medium should not be
heated. [Recipe: Book ref. 47, p. 666.] It is used e.g. for the
enrichment of salmonellae, although Proteus spp also grow well
in it.
tetrazoic Of a coccidian oocyst: containing four sporozoites per
sporocyst.
tetrazolium Tetrazolium salts e.g. nitroblue tetrazolium (NBT),
2,3,5-triphenyltetrazolium chloride (TTC, = tetrazolium red)
can be reduced to coloured formazan compounds, each salt
being reduced at a specific REDOX POTENTIAL. Tetrazolium salts
have a wide range of applications as redox indicator dyes. For
example, they may be used to demonstrate reducing microenvironments generated as a result of microbial activity: e.g., regions
of concentrated bacterial growth on the surfaces of meat or other
foods may be demonstrated by the development of a colour in
these regions following treatment with a tetrazolium salt solution. (Reduction of tetrazolium salts may be prevented by low
pH and hence may not occur in the presence of fermentative
organisms.) NBT reduction in the cytoplasm of NEUTROPHILS
(resulting in the formation of bluish-black granules) is indicative of a normal metabolic burst associated with PHAGOCYTOSIS,
and is used in a test for normal neutrophil function [test: Book
ref. 53, pp. 12551256]. TTC is used in commercial kits for the
diagnosis of bacteriuria, TTC reduction being taken as indicative
of the presence of significant numbers of actively metabolizing
bacteria.
tetronomycin See MACROTETRALIDES.
tetrose A 4-carbon sugar (e.g. ERYTHROSE).
Texas fever Syn. REDWATER FEVER.
Texas red Sulphorhodamine 101 acid chloride: a FLUOROCHROME
(excitation at ca. 568 nm) used e.g. in FLOW CYTOMETRY.
Tex-KL bacterium Legionella dumoffii.
textile spoilage Textiles made from vegetable (cellulosic) fibres
e.g. cotton, linen, hessian (cf. RETTING) are susceptible to attack
by a range of cellulolytic fungi (e.g. Aspergillus spp, Chaetomium
globosum, Cladosporium herbarum), especially under damp
conditions, resulting in loss of strength and flexibility of the fabric,
odour production, discoloration, etc. Zalerion spp can cause
rotting of twines and ropes exposed to seawater. Preservatives
for textiles (usually for outdoor use) include e.g. copper (or
zinc) naphthenate, copperoxine, cuprammonium hydroxide,
dichlorophane, SALICYLANILIDES. (See also WOOL SPOILAGE.)
Textularia See FORAMINIFERIDA.
Textulariina See FORAMINIFERIDA.
TF0 F1 H+ -ATPase See PROTON ATPASE.
TFT TRIFLUOROTHYMIDINE.
TGE TRANSMISSIBLE GASTROENTERITIS.
Th (TH ) (immunol.) Helper T cell (see T LYMPHOCYTE).
Th1 T cells See T LYMPHOCYTE.
Th2 T cells See T LYMPHOCYTE.
Thalassicolla See RADIOLARIA.
Thalassiophyllum See PHAEOPHYTA.
Thalassiosira See DIATOMS.
Thermoactinomyces
thalidomide (as therapy for mycobacterial and HIV infections)
See INTERFERONS.
thallic conidiogenesis See CONIDIUM.
thalline (1) Of or pertaining to a THALLUS. (2) Syn. SOMATIC
(sense 1).
thalline margin (excipulum thallinum) (lichenol.) In a LECANORINE APOTHECIUM: lichenized tissue (i.e., tissue containing both
algal and fungal cells) external to (surrounding, and sometimes
obscuring) the PROPER MARGIN; the thalline margin is generally
the same colour as the thallus, but may differ in colour from the
hymenial disc.
thallium salts (inhibitory action) Low concentrations of thallium
salts (e.g. 0.01% thallous acetate) inhibit the growth of many
species of bacteria. Some species of Mycoplasma are not
inhibited, and thallous acetate is used in a selective medium for
the primary isolation of these organisms. (Thallium salts inhibit
the growth of M. genitalium, some strains of M. hominis, and
the related organism, Ureaplasma urealyticum.)
Thallobacteria A proposed class of bacteria (division FIRMICUTES) comprising branching, thread-like organisms (ACTINOMYCETES and related organisms) [Book ref. 22, p. 33]. (cf. e.g.
THERMOACTINOMYCES.)
Thallophyta A division of the plant kingdom containing those
organisms whose vegetative form is a thallus, i.e., the fungi,
algae etc.
thallose Consisting of or resembling a thallus.
thallospore (mycol.) Any SPORE formed by fragmentation of part
or all of a fungal thallus e.g. an ARTHROSPORE, CHLAMYDOSPORE
or OIDIUM.
thallus A vegetative form of an organism which is not differentiated into stem and leaves, as in fungi, algae and lichens.
THAM See TRIS.
Thamnidiaceae See MUCORALES.
Thamnidium See MUCORALES.
Thamnocephalis See MUCORALES.
Thamnolia A genus of fruticose LICHENS; photobiont: a green
alga. The thallus is hollow and may be erect or prostrate; fruiting
structures are unknown.
Thanatephorus See TULASNELLALES.
Thauera selenatis See SELENATE RESPIRATION.
ThayerMartin agar (VCN agar) An enriched growth medium
containing vancomycin, colistin and nystatin; it is used for the
selective culture of Neisseria spp from swabs taken e.g. from
the genitourinary tract. For culture of rectal swabs, trimethoprim
may be added to suppress swarming by Proteus spp. [Recipe:
Book ref. 2, p. 138.]
theca (1) In certain algae of the Chlorophyta: a type of cell
wall which lacks the microfibrillar structure typical of a
true algal CELL WALL, being composed of very small, more or
less isodiametric units or scales; such thecae appear to have
evolved as modifications of scaly coverings, and occur in certain
flagellates (e.g. TETRASELMIS). [Book ref. 123, p. 31.]
(2) See DINOFLAGELLATES.
Thecamoeba See AMOEBIDA.
thecate Possessing a THECA.
thecium An ambiguous term which can refer e.g. to the HYMENIUM of an ascomycete or to the entire ascocarp.
Theileria A genus of protozoa (subclass PIROPLASMASINA) parasitic in animals and transmitted by ticks (see EAST COAST FEVER
for life cycle); Theileria spp infect both red and white blood
cells of the vertebrate host (cf. BABESIA). The cells resemble
those of Babesia but are typically smaller. [Characterization of
some East African Theileria species by isoenzyme analysis: IJP
(1985) 15 271276.]
Thermoascus
thermolysin A heat-stable, neutral metallo-PROTEASE (EC
3.4.24.4) produced by a strain of Bacillus stearothermophilus
(B. thermoproteolyticus). It is the most heat-stable protease
available commercially, retaining 50% activity after 1 hour at
80 C. Thermolysin contains zinc and four Ca2+ ions/molecule.
It has a broad specificity.
Thermomicrobium A genus (incertae sedis) of aerobic, catalasepositive, chemoorganotrophic, thermophilic, Gram-negative
bacteria which occur e.g. in hot springs. Cells: non-motile,
pleomorphic, pink-pigmented rods, ca. 1.31.8 3.06.0 m.
Optimum growth temperature: 7075 C; optimum pH: 8.28.5.
GC%: 64. Type species: T. roseum. [Book ref. 22, pp. 338
339.]
Thermomonospora A genus of (typically) thermophilic bacteria (order ACTINOMYCETALES, wall type III) which occur e.g.
in soil and composts. The organisms form branching substrate and aerial mycelium; of the five recognized species,
T. alba, T. curvata, T. fusca and T. mesophila form white aerial
mycelium, while T. chromogena forms yellowish-brown aerial
mycelium. Spores are borne singly at the ends of short branched
or unbranched sporophores on the aerial hyphae (or, in at least
T. fusca, on both aerial and substrate mycelium). The organisms are metabolically versatile e.g. T. alba and T. curvata
can degrade agar, cellulose, and keratin, while T. alba can
also degrade pectin. Type species: T. curvata. [Book ref. 73,
pp. 119121; taxonomy and identification: JGM (1984) 130
525.] (cf. ACTINOBIFIDA.)
Thermomyces See HYPHOMYCETES; see also COMPOSTING.
thermonuclease See DEOXYRIBONUCLEASE.
thermophile An organism whose optimum growth temperature
is >45 C; this definition is widely used [see e.g. Book ref. 45,
p. 236, and Book ref. 196, p. 40] and is compatible with the definition of MESOPHILE. (See also PSYCHROPHILE.) Many published
ad hoc definitions of thermophile are mutually incompatible,
often because a given definition may be applicable in only a
limited context; moreover, such definitions are frequently incompatible with the generally accepted upper limit of mesophile.
Thermophiles occur e.g. in hot springs and other habitats (see
e.g. COMPOSTING, LEACHING, HYDROTHERMAL VENT); they include
e.g. species of METHANOCOCCUS, PYRODICTIUM, SULFOLOBUS,
THERMOBACTEROIDES, THERMOFILUM, THERMOMICROBIUM, THERMOPLASMA, THERMOPROTEUS, THERMOTHRIX and THERMUS.
A super-thermophile archaean, designated strain 121, has
been cultured from samples taken from a HYDROTHERMAL VENT;
it grows at 85121 C [Science (2003) 301 934].
(See also CALDOACTIVE.)
Thermoplasma A genus of aerobic, heterotrophic prokaryotes
(order THERMOPLASMALES, formerly class MOLLICUTES) which
occur e.g. in hot springs and self-heating coal refuse piles.
T. acidophilum grows on yeast extract at 5064 C at a pH of
0.83.0. Cells: pleomorphic cocci, ca. 0.10.3 m diameter, to
filamentous. GC%: ca. 46. [Book ref. 157, pp. 8891.]
Thermoplasmales An order of aerobic, thermophilic prokaryotes
of the domain ARCHAEA (formerly Archaebacteria) characterized
by the absence of a cell wall. One genus: THERMOPLASMA.
Thermoproteales An order of thermophilic, anaerobic sulphurdependent prokaryotes (domain ARCHAEA, formerly Archaebacteria) which occur e.g. in hot springs; growth is typically
chemolithoautotrophic and/or chemolithoheterotrophic. Cells:
cocci, rods or irregularly shaped forms, the cell wall typically
being a detergent-resistant S LAYER. Genera: DESULFUROCOCCUS,
PYRODICTIUM, THERMOCOCCUS, THERMODISCUS, THERMOFILUM and
THERMOPROTEUS.
Thiobacillus
positive charge and is usually supplied commercially as thiamine
chloride hydrochloride (thiamine hydrochloride). The coenzyme form is thiamine pyrophosphate (TPP, cocarboxylase).
TPP functions in decarboxylation reactions (e.g. pyruvate
acetaldehyde); in oxidative decarboxylations e.g. (in conjunction with LIPOIC ACID) of pyruvate and 2-oxoglutarate [see
Appendix II(a)]; in a-ketol formation e.g. acetoin formation
[Appendices III(c) and III(f)]; in transketolase and phosphoketolase reactions [Appendices I(b) and III(b), respectively]; etc.
Thermoproteus
NH2
N
H3C
S
CH2
N+
CH3
CH2
CH2OH
THIAMINE
Thiocapsa
up to 40 nm in diameter. Oligomerization is temperaturedependent, activity being reduced at low temperatures.
Studies with animal models have indicated that at least some
of the toxins (e.g. pneumolysin) can contribute to virulence.
The thiol-activated cytolysins include:
alveolysin (Bacillus alvei )
bifermentolysin (Clostridium bifermentans)
botulinolysin (C. botulinum)
cereolysin (B. cereus)
chauveolysin (d-toxin of C. chauvoei )
histolyticolysin (e-toxin of C. histolyticum)
ivanolysin (Listeria ivanovii )
laterosporolysin (B. laterosporus)
listeriolysin (L. monocytogenes)
oedematolysin (d-toxin of C. novyi )
perfringolysin (q-toxin of C. perfringens)
pneumolysin (Streptococcus pneumoniae)
seeligerolysin (L. seeligeri )
septicolysin (d-toxin of C. septicum)
sordelliolysin (C. sordelli )
STREPTOLYSIN O (q.v.)
tetanolysin (C. tetani )
thuringiolysin (B. thuringiensis)
[Thiol-activated cytolysins: RMM (1996) 7 221229.]
thiol protease See PROTEASES.
thiomersal (merthiolate; thimerosal) Sodium ethylmercurithiosalicylate, C2 H5 .Hg.S.C6 H4 .COONa. An antibacterial and antifungal agent used as a preservative e.g. in biological laboratory
reagents; it is effective in low concentrations (e.g. 0.010.02%).
Thiomicrospira A genus of bacteria which occur e.g. in estuarine
muds and in the vicinity of HYDROTHERMAL VENTS. Cells: curved
or spiral rods; many strains are motile by means of a single
polar flagellum. The organisms resemble THIOBACILLUS in general physiology. T. denitrificans and T. pelophila are both obligate chemolithotrophs. [Culture: Book ref. 45, pp. 10231036;
T. crunogena, an obligately chemolithoautotrophic species from
a hydrothermal vent: IJSB (1985) 35 422424.]
thionin (Lauths violet) A bluepurple dye structurally related
to METHYLENE BLUE. (See also BRUCELLA.)
Thiopedia See CHROMATIACEAE and COENOBIUM.
thiopeptin A peptide antibiotic related to THIOSTREPTON; it is
active against e.g. Streptococcus bovis. Thiopeptin inhibits
experimentally-induced lactic ACIDOSIS in ruminants.
thiophanate-methyl (1,2-bis(3-methoxycarbonyl-2-thioureido)
benzene) An agricultural antifungal agent (see BENZIMIDAZOLES) which is effective e.g. against Rhizoctonia solani infections in seedlings, Pyricularia oryzae in rice, eyespot and Rhynchosporium infection in cereals, and black spot of roses; it also
has some effect in controlling clubroot in crucifers.
thiophene-2-carboxylic acid hydrazide test Syn. T2H TEST.
a-thiophosphoryl dATP See SDA.
Thioploca A genus of GLIDING BACTERIA (see CYTOPHAGALES)
which occur e.g. in sulphide-containing muds (freshwater to
marine). The organisms occur as sheathed fascicles, each fascicle
(macroscopic in some species) consisting of a longitudinally
arranged bundle of filaments; individual filaments (ca. 110 m
wide; wider in marine species) can glide in the sheath and
emerge from it. In at least some species metabolism involves
oxidation of sulphide. Sulphur is deposited intracellularly. Type
species: T. schmidlei. Other species: e.g. T. ingrica from lake
sediments [IJSB (1984) 34 344345], T. araucae, T. chileae
(marine benthic species) [IJSB (1984) 34 414418].
T. denitrificans. Electron donors: e.g. sulphide and thiosulphate. Under aerobic conditions oxygen is the electron acceptor;
anaerobically, nitrate, nitrite or nitrous oxide can function as
electron acceptor, and is reduced to nitrogen. Optimum pH: 68.
T. ferrooxidans. Aerobic; growth also occurs anaerobically
with ferric ions as electron acceptor for the oxidation of
reduced sulphur compounds. Electron donors include sulphur,
thiosulphate, sulphide and ferrous ions. Capable of NITROGEN
FIXATION. Optimum growth temperature: ca. 20 C. Growth
occurs within the approximate pH range 1.46.0. (See also
LEACHING.) [Molecular genetics of T. ferrooxidans: MR (1994)
58 3955.]
T. thiooxidans. Electron donors include e.g. thiosulphate and
(particularly) elemental sulphur. Optimum pH: ca. 24; growth
occurs within the approximate range 0.56.0. Can cause RUBBER
SPOILAGE. (See also LEACHING.)
T. thioparus. Motile rods. Electron donors include sulphide
and thiosulphate; some strains can use thiocyanate (CNS ).
A sulphur-containing pellicle may be formed on thiosulphatecontaining liquid media. Nitrate is reduced to nitrite during
anaerobic growth. Optimum growth temperature: ca. 28 C.
Optimum pH: ca. 68; growth ceases below ca. pH 4.5.
T. versutus (formerly Thiobacillus A2). A species capable
of chemolithoautotrophic or mixotrophic growth. Oxidation of
organic substrates (but not inorganic sulphur compounds) can be
coupled to the reduction of nitrate.
Other species include T. intermedius and T. perometabolis
[IJSB (1984) 34 139144], T. acidophilus, T. neapolitanus,
T. novellus and T. organoparus.
[Media and culture: Book ref. 45, pp. 10231036.]
Thiocapsa A genus of photosynthetic bacteria (family CHROMATIACEAE). The cells are non-motile cocci; in addition to various
carotenoids, T. roseopersicina (1.23.0 m) contains Bchl a,
and T. pfennigii (ca. 1.5 m) contains Bchl b cell suspensions typically being reddish and orange-brown, respectively.
In T. pfennigii the pigments occur in tubular intracytoplasmic
membrane systems. Gas vacuoles are absent. T. roseopersicina
is moderately tolerant of organic pollution, and may give rise to
reddish blooms in sewage lagoons; it is capable of chemoorganotrophic growth under microaerobic conditions in the dark.
thioctic acid Syn. LIPOIC ACID.
Thiocystis See CHROMATIACEAE.
Thiodictyon See CHROMATIACEAE.
thioglycollate broth See e.g. BREWERS THIOGLYCOLLATE MEDIUM.
thiol-activated cytolysins (SH-activated cytolysins) A class of
cytolysins, formed by certain bacteria, which are active only in
the reduced state, and which can be (reversibly) activated by
thiols; the cytolytic activity of these toxins is confined to those
cells (including e.g. erythrocytes) whose cytoplasmic membrane
contains cholesterol. Thiol-activated cytolysins are formed by
species of the (Gram-positive) bacteria Bacillus, Clostridium,
Listeria and Streptococcus. (A thiol-activated cytolysin was
reported to be formed by the (Gram-negative) species Klebsiella
pneumoniae [CJM (1985) 31 297300].)
The thiol-activated cytolysins are proteins of 4760 kDa;
they are optimally active at similar values of pH and temperature, they cross-react serologically, and their haemolytic activity
is irreversibly lost in the presence of cholesterol or stereochemically related sterols.
The thiol-activated cytolysins are pore-forming agents. They
bind reversibly, in a temperature-independent manner, to
cholesterol-containing membranes, and oligomerize to form
(typically) ring-shaped formations (pores in the membrane) of
772
three-for-one model
seems to be derived from the oxidation of sulphide or thiosulphate; sulphur is deposited intracellularly. One strain of Thiothrix has been found to contain carboxysome-like structures,
suggesting that it may be autotrophic. [Review: ARM (1983) 37
354359.]
thiourea derivatives (as antimicrobial agents) Antimicrobial derivatives of thiourea, (NH2 )2 CS, include e.g. diphenylthiourea,
(C6 H5 NH)2 CS, which has been used as an antimycobacterial
agent, and the THIOSEMICARBAZONES.
Thiovulum A genus of bacteria (Proteobacteria) found e.g. in
marine habitats characterized by the simultaneous presence of
sulphide and oxygen; the organisms obtain energy by oxidizing
sulphide/sulphur, and typically form a whitish layer at the
interface of sulphidogenic sediments and oxygenated water.
Cells of the sole species, T. majus, are spherical, with a diameter
reported to range from 5 to 25 m; the (flagellate) organisms
can reach speeds of 600 m/second [Microbiology (1994) 140
31093116].
thiram (TMTD) TetramethylTHIURAM DISULPHIDE: (CH3 )2 .N.CS.
S.S.CS.N.(CH3 )2 ; an ANTIFUNGAL AGENT which is also active
against (mainly) Gram-positive bacteria. (cf. DMDC.) Thiram
has been used as an antiseptic in the topical treatment of
dermatophyte infections, and as an agricultural antifungal agent
(e.g. as a seed dressing, and for the control of apple scab, Botrytis
fruit rots, etc). Thiram (being insoluble in water) is used in
aqueous suspensions.
35 sequence See PROMOTER.
thistle mottle virus See CAULIMOVIRUSES.
thiuram disulphides These compounds (R2 .N.CS.S.S.CS.N.R2 )
are formed by the mild oxidation of DITHIOCARBAMATES. See e.g.
METIRAM and THIRAM.
Thogoto virus An unclassified virus (see ORTHOMYXOVIRIDAE)
which has been isolated from ticks and mammals; it has
been implicated in a severe human disease (optic neuritis,
meningoencephalitis) in Africa.
Thoma chamber See COUNTING CHAMBER.
thraustochytrids A category of eukaryotic organisms which
are generally classified together with the LABYRINTHULAS
(q.v.). (The thraustochytrids were formerly included within the
Oomycetes either as a family, Thraustochytriaceae, of the
Saprolegniales, or as a distinct order, Thraustochytriales.) The
organisms are widely distributed in marine and esturaine waters,
living apparently mainly as saprotrophs on algae, plants,
organic detritus, etc. The vegetative stage consists of a rounded
or oval, somewhat amoeboid cell from which arise ectoplasmic
filaments that branch and anastomose to form a rhizoid-like
ectoplasmic net. The net is produced from sagenogenetosomes
(sagenogens, bothrosomes) which are essentially similar to
those of labyrinthulas; it appears to function in adhesion and
nutrition (which is osmotrophic) and to some extent in motility,
but the cell does not move into the net (cf. LABYRINTHULAS).
The cell body serves as a sporangium which, in most species,
gives rise to laterally biflagellate zoospores resembling those of
LABYRINTHULAS (although apparently lacking an eyespot). Genera
include Aplanochytrium (which produces aplanospores instead of
zoospores), Japonochytrium, Labyrinthuloides, Schizochytrium
and Thraustochytrium.
Thraustochytrium See THRAUSTOCHYTRIDS.
three-component regulatory system See BACTERIOCINS.
three-for-one model (3-for-1 model) A model which describes
the mode in which newly synthesized PEPTIDOGLYCAN (q.v.) is
incorporated in the sacculus of a growing cell [Microbiology
(1996) 142 19111918].
(a)
(b)
(c)
THREE-FOR-ONE MODEL: incorporation of newly synthesized peptidoglycan in the sacculus of a growing cell of Escherichia coli (simplified
outline, diagrammatic). In PEPTIDOGLYCAN (q.v.), the glycan backbone chains are perpendicular to the long axis of the cell; the diagram shows an
end-on view of backbone chains (open circles) joined by peptide bridges (straight lines).
(a) A peptidoglycan monolayer; the monolayer is a stress-bearing structure and is under considerable tension. The chain in the centre
( ) a docking chain is to be replaced by three chains (hence 3-for-1).
(b) A triplet of three linked chains is located below (i.e. on the cytoplasmic side of) the peptidoglycan monolayer, with the flanking chains of
the triplet covalently bound either side of the docking chain; in this particular plane, a stem peptide from each flanking chain has bound to the
e-amino group of a dimeric peptide bridge to form a trimeric bridge (see legend to figure in entry PEPTIDOGLYCAN).
(c) The docking chain has been removed by enzymic action, and because of the tension in the monolayer the incoming triplet of chains
has taken up its position in the sacculus; note that this contributes to cell elongation. The model assumes that the central chain in the incoming
triplet will, when incorporated in the sacculus, function as a new docking chain; for this reason, the dimeric bridge to each flanking chain is
assumed to have a free e-amino group located in the stem peptide of the flanking chain.
For cell length to double during the cell cycle, the model assumes that (i) docking and non-docking chains alternate in the sacculus, and (ii)
only those docking chains which are present at the start of the new cell cycle will be replaced by an incoming triplet; that is, new docking
chains inserted during the current cell cycle will not be replaced until the next cell cycle. For this purpose, the growth mechanism must be
able to distinguish old from new docking chains. This is possible because newly synthesized peptidoglycan is linked to the sacculus solely
by tetra-tetra peptide bridges; it is therefore postulated that new chains (identified by their tetra-tetra links) are not recognized as docking
chains, but that, at the start of each new cell cycle, all tetra-tetra links will have been changed enzymically (by an LD-carboxypeptidase) to
tetra-tri links, and that this allows recognition of the functional docking chains.
Reproduced from Bacteria, 5th edition, Figure 3.1, page 42, Paul Singleton (1999) copyright John Wiley & Sons Ltd, UK (ISBN 0471988804)
with permission from the publisher.
timber spoilage
In a typical life cycle, a teliospore germinates to give rise to
an elongated, aseptate or uniseptate structure bearing an apical
tuft of eight or more thread-like basidiospores (sometimes called
primary sporidia or primary conidia); in e.g. T. caries (which
exhibits HETEROTHALLISM) the basidiospores on a given structure
are of two different mating types. While still attached, the
basidiospores conjugate in pairs, giving rise to H-shaped forms
within which plasmogamy occurs; subsequently, each (detached)
H-shaped binucleate form, or mycelium derived from it, gives
rise to binucleate ballistoconidia (sometimes called secondary
sporidia or secondary conidia). The conidia germinate to form
dikaryotic hyphae which initiate infection of a fresh host and
subsequently give rise to teliospores.
Tilletiaceae See USTILAGINALES.
tilmicosin A MACROLIDE ANTIBIOTIC which has been used e.g.
against Mycoplasma bovis in the treatment of CALF PNEUMONIA;
in vitro tests on field isolates of M. bovis indicate that significant
levels of resistance have developed against tilmicosin [VR
(2000) 146 745747].
Tilopteris See PHAEOPHYTA.
tilorone
(2,7-bis-[2-(diethylamino)ethoxyl]-9-fluorenone) An
antiviral, antitumour agent which seems to (a) induce INTERFERON synthesis, and (b) interfere directly with virus expression
by functioning as an INTERCALATING AGENT (f ca. 13 ) with a
preference for AT-rich regions of dsDNA.
Tilsit cheese See CHEESE-MAKING.
Tilt See PROPICONAZOLE.
timber decay See TIMBER SPOILAGE and TREE DISEASES.
timber preservation The seasoning (i.e. drying) of timber
renders it less susceptible to fungal attack (see TIMBER SPOILAGE),
and may facilitate penetration by chemical preservatives; once
dried, timber can be preserved by e.g. preventing the access of
air and moisture by the use of sealants or paint films (see also
PAINT SPOILAGE). In some cases (e.g. elm wood) decay can be
inhibited by waterlogging which limits the supply of oxygen to
potential spoilage fungi.
Decay of timber may also be prevented or delayed by the
use of PRESERVATIVES e.g. CREOSOTE, sodium fluoride, pentachlorophenol, borates (alone or with QACs), copper naphthenate, and tributyl tin oxide (alone or with QACs). Most of
these substances are inherently fungitoxic, but tributyl tin oxide
(TBTO) inhibits fungal attack by binding strongly to cellulose,
rendering it insusceptible to fungal CELLULASES; wood treated
with TBTO may still be susceptible to lignin-utilizing WHITE
ROT fungi unless TBTO is used in conjunction with e.g. a phenolic preservative to protect the lignin. The control of SOFT
ROT can be achieved only by the use of preservatives which
penetrate into the cell walls of the wood. Preservatives may
be applied either as surface coatings or by the use of specialized procedures (see e.g. BETHELL PROCESS; BOUCHERIE PROCESS;
SAUGKAPPE PROCESS). Aqueous preservatives may be retained
in treated timbers e.g. by the formation of insoluble precipitates;
the insolubility of some preservatives prevents leaching under
damp or wet conditions. (Certain types of wood contain natural
fungitoxic substances e.g. PINOSYLVIN in pine, TANNINS in oak,
THUJAPLICINS in Western Red Cedar.) (See also HETEROBASIDION.)
Decay of chemically treated timber may occur e.g. through
splitting which permits fungal penetration through a treated
zone. Rhizomorphs may enable a fungus to cross treated (or nonnutrient) zones (see e.g. DRY ROT), while some fungi can detoxify
copper preservatives by converting them to copper oxalate.
timber spoilage Microbial spoilage of timber is caused primarily
by fungi particularly basidiomycetes and involves decay
timber staining
(see e.g. BROWN ROT, DRY ROT, POCKET ROT, SOFT ROT, WET
and WHITE ROT) and/or staining (see TIMBER STAINING).
Commonly, only wood having a moisture content greater than
ca. 20% is susceptible to fungal attack (cf. DRY ROT); the moisture
content is calculated as the weight of water in a sample of
timber divided by the dry weight of that sample. In fallen
or freshly felled timber the sapwood is particularly vulnerable
to SAP-STAIN and early decay by any of a range of fungi;
thus e.g. fallen birch branches rapidly succumb to a brown
cubical rot (caused by e.g. Piptoporus betulinus) or to a soft
white fibrous rot (caused e.g. by Heterobasidion annosum see
HETEROBASIDION). Timber may also support a surface growth of
non-cellulolytic, non-lignolytic ascomycetes and deuteromycetes
(cf. SOFT ROT (1)); such growth generally causes little or no
damage to the timber. Fungi of importance in the decay of
domestic and industrial timbers include e.g. Serpula lacrymans
(see DRY ROT) and Coniophora puteana (see WET ROT); Lentinus
lepideus is moderately resistant to creosote and can cause a
brown rot in e.g. railway sleepers. (See also PAPER SPOILAGE;
TIMBER PRESERVATION; TREE DISEASES.)
timber staining (by fungi) Various wood-infecting fungi cause
discoloration in felled timber and in standing trees; some
infections are superficial, but in others the fungus grows into
the timber or is carried in by wood-boring beetles. Superficial
staining can be caused by a range of fungi (e.g. species of
Alternaria, Fusarium, Penicillium) and typically does not affect
the strength or value of the timber; deep staining may weaken
the timber (see e.g. BROWN OAK). Staining may be due to the
production of a fungal pigment or to an optical effect (see BLUESTAIN). (See also GREEN OAK; TIMBER PRESERVATION.)
Timentin A composite antibiotic consisting of ticarcillin (see
PENICILLINS) and CLAVULANIC ACID. [Clinical evaluation: Am.
J. Med. (1985) 79 Supplement 5B 1196; laboratory and
clinical perspective: JAC (1986) 17 Supplement C 1244.] (cf.
AUGMENTIN.)
timothy-grass bacillus Mycobacterium phlei.
tin (as an antimicrobial agent) Tin is a HEAVY METAL which, in
elemental or compound form, can exert antimicrobial activity.
The presence of metallic tin has been reported to inhibit growth
and toxin production by Clostridium botulinum in food contained
in tin-plate cans [cited in Book ref. 35, p. 282]. (If the inside
of a can is significantly de-tinned e.g. by CURING salts, or by
certain acidic fruits the underlying steel may rapidly corrode
and give rise to a HYDROGEN SWELL.)
Organotins (i.e. tin-containing organic compounds) are typically more active than inorganic compounds of tin trialkyltins
(e.g. TBTO) being among the most effective. (See also FENTIN.)
Trisubstituted organotins exhibit microbistatic activity at low
concentrations apparently by inhibiting ATP synthesis; at high
concentrations they can be microbicidal, possibly by disrupting
the cytoplasmic membrane.
tinangaja disease A disease of coconut palms which occurs on
the island of Guam; it is apparently caused by the COCONUT
CADANG-CADANG VIROID.
tincture of iodine See IODINE (a).
tinder fungus Fomes fomentarius.
tinea See RINGWORM. (See also e.g. FAVUS; PITYRIASIS NIGRA;
PITYRIASIS VERSICOLOR.)
tinidazole See NITROIMIDAZOLES.
Tinopal AN A FLUORESCENT BRIGHTENER used e.g. as a selective
antibacterial agent; in e.g. Escherichia coli it apparently inhibits
RNA polymerase [JGM (1984) 130 19992005]. [Use for
distinguishing phytopathogenic from saprotrophic Pseudomonas
spp: JAB (1985) 58 283292.]
ROT,
776
TMA
titer See TITRE.
titration (mol. biol.) Concentration-dependent interaction between a regulatory molecule and other molecule(s) or specific
nucleotide sequence(s) by means of which the level of activity
of the regulatory molecule is controlled. (See e.g. F PLASMID
(replication).)
titre (titer) (serol., virol.) A numerical expression for the concentration of specific antibodies, antigens, virions etc in a given
sample. If the titre of antibodies or antigens is determined by
an END-POINT TITRATION, the titre is equal, numerically, to the
dilution factor of the highest dilution of sample giving a positive serological reaction. For example, if the end-point reaction
mixture consisted of a 1/200 dilution of serum (antibody) and
an equal volume of antigen, the titre of antibody can be given
as 200 (initial serum dilution) or 400 (final serum dilution);
these titres may, alternatively, be quoted as 1/200 and 1/400,
respectively.
Virus titres may be determined e.g. by the PLAQUE ASSAY
method (see also END-POINT DILUTION ASSAY).
TK THYMIDINE KINASE.
TLC Thin-layer CHROMATOGRAPHY.
Tm (Tm ) See THERMAL MELTING PROFILE.
TMA Trimethylamine (see e.g. FISH SPOILAGE).
TMA (transcription-mediated amplification) A method used for
the isothermal amplification of RNA target sequences; the
principle of TMA is the same as that of NASBA (q.v.) one
practical difference being that, in the commercial applications
of TMA, use is made of the RNase H activity of reverse
transcriptase, so that only two enzymes are used.
Commercial TMA- and NASBA-based tests differ also in
the way in which amplified target sequences are detected.
In TMA-based tests, the targets are detected by a so-called
hybridization protection assay (HPA). HPA involves the use
of DNA probes labelled with acridinium ester. After allowing
time for probetarget hybridization, an added reagent hydrolyses
the acridinium ester label on all unbound probes the label
on bound probes being protected as a consequence of its
location within the probetarget duplex; subsequent addition
of other reagents elicits CHEMILUMINESCENCE from the bound
probes emitted light being measured by a luminometer in
relative light units (RLUs).
Commercial applications of TMA include several diagnostic
tests one of which, the amplified Mycobacterium tuberculosis direct test (AMTDT; Gen-Probe, San Diego, USA), was
approved by the U.S. Food & Drug Administration (FDA)
for detection of Mycobacterium tuberculosis in (smear-positive)
respiratory specimens (e.g. sputa). A new-format enhanced
AMTDT, which uses a larger volume of sample, was approved
by the FDA in 1998.
A TMA-based test for Chlamydia trachomatis in urogenital
specimens was approved by the FDA in 1996; the principle of
this test (AMP CT) is identical to that of the AMTDT.
[Evaluation of AMP CT for the detection of Chlamydia trachomatis in a high-risk population of women: JCM
(1997) 35 676678. Evaluation of AMTDT for non-respiratory
specimens: JCM (1997) 35 307310. Comparison of original and enhanced versions of AMTDT for respiratory and
non-respiratory specimens: JCM (1998) 36 684689. Evaluation of enhanced AMTDT for rapid diagnosis of pulmonary
tuberculosis in a high-risk prison population: JCM (1999) 37
14191425. False-positive results with AMTDT in patients with
Mycobacterium avium and M. kansasii infections: JCM (1999)
37 175178.]
TMAO
and IS50 R) that differ slightly from one another. Each IS50
sequence is flanked by a pair of 19-bp sequences referred to as
the outer end (OE) and inner end (IE); the two OE sequences
thus form the two ends of the transposon.
IS50 R encodes two proteins: P1 (a cis-acting transposase,
Tnp) and P2 (an inhibitor of the transposase, Inh) P2 being
encoded by the same reading frame as P1 but lacking the Nterminal 55 amino acids. (IS50 L encodes two corresponding
proteins, P3 and P4; however, IS50 L contains an ochre codon
so that P3 and P4 are non-functional proteins.)
Tnp can catalyse transposition of (i) the entire transposon
(Tn5 ) or (ii) IS50 ; transposition of Tn5 involves the two OE
sites, whereas transposition of IS50 involves one OE site and
one IE site.
Tnp is characterized by a low level of activity which is
further down-regulated by Inh; the relative levels of Tnp and
Inh influence the frequency of transposition. In vivo, host factors
tend to favour transposition from the OE sites (in preference
to the IE sites). Other regulatory factors in vivo include
dam methylation (see DAM GENE) which negatively affects the
function of the P1 promoter (and also results e.g. in coupling
transposition to DNA replication).
[Tn5 (review): ARM (1993) 47 945963.]
Early studies suggested that transposition of Tn5 may involve
a cut-and-paste (rather than a replicative) mechanism (see
TRANSPOSABLE ELEMENT) [CSHSQB (1984) 49 215226], but
subsequent work suggested the involvement of cointegrates (i.e.
a replicative mechanism) [JMB (1986) 191 7584]. However,
more recent evidence favours a cut-and-paste model [JBC (1998)
273 73677374].
The latter study [JBC (1998) 273 73677374] demonstrated
that transposition could be achieved in an in vitro system consisting of: (i) transposase, (ii) DNA flanked by OE sequences,
and (iii) target DNA. Such in vitro transposition is optimized by
a hyperactive form of transposase transcribed from IS50 R containing three mutations one of which blocks transcription of
the inhibitor (Inh) while another enhances the binding of transposase to OE sequences.
Tn7 A TRANSPOSON which can insert into the chromosome of
Escherichia coli with a high degree of target specificity; the
target site is designated attTn7. Insertion of Tn7 involves several
Tn7-encoded proteins: TnsA, TnsB, TnsC and TnsD; TnsA and
TnsB jointly provide transposase activity. Initially, TnsD binds
to attTn7 in a sequence-specific way, and such binding distorts
the 5 end of the binding site; it has been suggested that this
distortion of DNA acts as a signal for the recruitment of TnsC
to the site [EMBO (2001) 20 924932].
A second, distinct pathway of transposition of Tn7 involves
the transposon-encoded TnsA, TnsB, TnsC and TnsE; TnsE,
which binds DNA in a structure-dependent way, promotes insertion of Tn7 into (i) certain plasmids, and (ii) the chromosome of
E. coli at sites proximal to double-stranded breaks in DNA and
also at locations where DNA replication terminates [GD (2001)
15 737747].
Tn9 A 2638-bp composite TRANSPOSON which includes terminal,
directly repeated IS1 elements and a gene (cat) for resistance
to CHLORAMPHENICOL (cat encodes chloramphenicol acetyltransferase an enzyme which also inactivates fusidic acid). Tn9
apparently transposes by a replicative process involving cointegrate formation, recA function being necessary for cointegrate resolution [JMB (1986) 191 7584]. (cf. Tn3 and Tn5.)
Tn9 occurs e.g. in the R plasmid pSM14 (= R14), a plasmid
which also contains Tn10. Tn9-derived chloramphenicol resistance from Gram-negative bacteria can be cloned in, but not
TNF
phenotypically expressed in, Bacillus subtilis [PNAS (1982) 79
58865890]. (See also IS1.)
Tn10 A 9.3-kb composite TRANSPOSON which carries a gene for
tetracycline resistance; Tn10 occurs e.g. in the transmissible
plasmid R100 (= R222). The mechanism of Tn10 transposition
is distinct from that of Tn3 (q.v.); it apparently involves a nonreplicative cut-and-paste mechanism in which excision of the
transposon from the donor molecule (by double-stranded breaks
at each end) is followed by insertion of the transposon into
the new target site. The remainder of the donor molecule is
probably lost (donor-suicide model). [Genetic evidence for
non-replicative Tn10 transposition: Cell (1986) 45 801815.]
The two ends of Tn10 are IS elements (IS10, 1.4 kb) in
opposite orientation; the two IS10 elements are similar but not
identical, and are designated IS10-Right (IS10-R) and IS10Left (IS10-L). IS10-R encodes at least one protein (transposase)
which acts at the ends of Tn10 and is necessary for its
transposition; the transposase is apparently preferentially cisacting, possibly migrating along the DNA molecule rather
than being freely diffusible in the cell cytoplasm. IS10-R
can promote normal levels of transposition (e.g. ca. 107
transpositions/TE/bacterial generation) even when IS10-L is
inactive; however, IS10-L is functionally defective and can
provide only ca. 110% of the transpositional activity of IS10-R.
Insertion of Tn10 into a new target site presumably recognized
by the IS10-R transposase results in the duplication of a 9-bp
target sequence. The preferred (hot-spot) target site for Tn10
contains a symmetrical 6-bp sequence within the 9-bp sequence
(NGCTNAGCN) duplicated during insertion; insertion can also
occur, less efficiently, at many other sites, with concomitant
duplication of a different 9-bp sequence. (See also DAM GENE
and MULTICOPY INHIBITION.)
Tn21 A 19.3-kb Tn3-like transposon (see Tn3) present e.g. in
plasmid R100 from Shigella flexneri ; it encodes resistance to
sulphonamides, streptomycin and mercuric ions. Tn21 transposition is regulated by a modulator protein encoded by a gene
(tnpM) located upstream of the Tn21 IRS. The tnpA, tnpR and
tnpM genes are all transcribed in the same direction (cf. Tn3).
The Tn21 modulator apparently enhances Tn21 transposition and
suppresses cointegrate resolution by Tn21 resolvase. A sequence
homologous to the Tn21 tnpM gene has been observed in an
analogous site in Tn501. [Cell (1985) 42 629638.]
Tn501 An 8.2-kb Tn3-like transposon (see Tn3) from Pseudomonas spp (plasmid pUS1); it encodes resistance to mercury.
The frequency of transposition and efficiency of cointegrate resolution are both substantially increased in the presence of low
levels of mercury, suggesting that the tnpA and tnpR genes can
be transcribed from the same promoter as the inducible gene for
mercury resistance. Tn501 may encode a modulator protein similar to that of Tn21 (q.v.). Tn501 provides hot-spots for Tn3
insertion.
Tn551 See Tn3.
Tn554 A site-specific, repressor-controlled TRANSPOSON from
Staphylococcus aureus; it carries (inducible) genes for resistance
to erythromycin and spectinomycin.
Tn916 See CONJUGATIVE TRANSPOSITION.
Tn925 See CONJUGATIVE TRANSPOSITION.
Tn951 A defective transposon of the Tn3 group (see Tn3) which
encodes genes for lactose metabolism (lacZ and lacY); its ends
are perfect inverted repeats (40 bp), but it apparently lacks
genes for its transposition transposition requiring Tn3-encoded
transposase and resolvase. (cf. IS101.) Tn951 contains an IS1
sequence [MGG (1980) 178 367374].
tnpA gene
TMV infects tobacco (Nicotiana tabacum) and other plants. The
common, Vulgare or field strain (U1 strain) usually causes
a systemic disease of tobacco in which leaves are distorted,
blistered, and marked with a mosaic of light and dark green
patches; intracellular crystalline arrays of virus particles are
commonly visible by light microscopy. Other TMV strains may
affect other plants (e.g. strain Cc affects legumes, TMV-L affects
tomatoes). (See also PATHOGENESIS-RELATED PROTEINS.) TMV is
transmitted mechanically; it may remain infective for a year or
more in soil or dried leaf tissue. The virions may be inactivated
e.g. at pH <3 or >8 or by formaldehyde, iodine, etc; TIP:
ca. 95 C. Preparations of TMV may be obtained from plant
tissues e.g. by (NH4 )2 SO4 precipitation followed by differential
centrifugation.
The TMV ssRNA genome is ca. 6400 nucleotides long
[sequence: PNAS (1982) 79 58185822] and is capped at the
5 end (sequence: m7 G5 ppp5 Gp) but is not polyadenylated.
The genomic RNA can serve as mRNA for a protein of MWt
ca. 130000 (130 K) and another, produced by readthrough,
of MWt ca. 180000 (180 K); however, it cannot function as
messenger for the synthesis of e.g. coat protein. Other genes are
expressed during infection by the formation of monocistronic, 3 coterminal SUBGENOMIC MRNAS, including one (LMC) encoding
the 17.5 K coat protein and another (I2 ) encoding a 30 K protein.
(Other putative subgenomic mRNAs may be artefacts generated
during electrophoresis [Book ref. 80, pp. 6972].) The 30 K
protein has been detected in infected protoplasts [Virol. (1984)
132 7178]; it may be involved in the cell-to-cell transport of
the virus in an infected plant. The functions of the two large
proteins are unknown.
Several dsRNA molecules including dsRNAs corresponding to the genomic, I2 and LMC RNAs have been detected in
plant tissues infected with TMV; these are presumably intermediates in genome replication and/or mRNA synthesis processes
which appear to occur by different mechanisms [Book ref. 80,
pp. 8487].
TMV assembly apparently occurs in the plant cell cytoplasm,
although it has been suggested that some TMV assembly may
occur in chloroplasts since transcripts of ctDNA have been
detected in purified TMV virions [Book ref. 80, pp. 7379].
Initiation of TMV assembly occurs by interaction between ringshaped aggregates (discs) of coat protein (each disc consisting
of two layers of 17 subunits) and a unique internal nucleation
site in the RNA: a hairpin region ca. 900 nucleotides from the
3 end in the common strain of TMV. (Any RNA including
e.g. subgenomic RNAs containing this site may be packaged
into virions.) The discs apparently assume a helical form on
interaction with the RNA, and assembly (elongation) then
proceeds in both directions (but much more rapidly in the 3 -to5 direction) from the nucleation site. [Review of structure and
assembly: JGV (1984) 65 253279.]
tobacco necrosis virus (TNV) A PLANT VIRUS which can infect
a range of angiosperms; transmission occurs via Olpidium spp
and can occur mechanically under experimental conditions.
Symptoms of TNV infection range from severe necrosis (e.g.
in Augusta disease of tulips) to local necrotic leaf lesions (e.g.
in tobacco seedlings). Virion: icosahedral, ca. 28 nm diam.,
containing one polypeptide species (MWt ca. 22600); genome:
a single molecule of linear positive-sense ssRNA (MWt ca.
1.31.6 106 ) with the 5 -terminal sequence: ppApGpU. . . .
TNV-infected plant cells may also contain a SATELLITE VIRUS:
an icosahedral, ssRNA-containing virus [structure: JMB (1982)
159 93108] which is completely dependent on the presence of
[TIM (1998) 6 228233]. (See also DISSEMINATED INTRAVASCULAR COAGULATION and other cytokine-associated conditions listed
under CYTOKINES.)
In some individuals, susceptibility to a severe form of
MALARIA has been found to correlate with a variant form of
the TNF-a promoter [Nature (1994) 371 508510], and an
increased susceptibility to endotoxic shock appears to correlate
with enhanced synthesis of TNF [JAMA (1999) 282 561568].
The apparent link between levels of TNF and pathogenesis has
suggested that benefit may be obtained, in certain cases, from
the use of ligands that sequester TNF and prevent its binding
to specific cell-surface receptors; such anti-TNF ligands include
etanercept and the monoclonal antibody infliximab.
TNF-a exists in both soluble (secreted) and membraneassociated forms, both forms being active.
TNF-b (also called lymphotoxin a) is produced by activated
lymphocytes, and is characteristic of the Th1 subset of T
cells. TNF-b resembles TNF-a in its activities many of which
coincide with the activities of INTERLEUKIN-1; unlike IL-1,
however, TNF can trigger apoptosis in a target cell.
The cell-surface receptors of tumour necrosis factor are
designated p55 (= CD120a) and p75 (= CD120b) and they
occur on a wide range of cells. Each type of receptor can
apparently serve as a binding site for both forms of TNF;
however, the two receptors may have distinct roles in TNF
activity, and p75 may have a subordinate role. Following
endotoxaemia, the peripheral circulation contains raised levels
of soluble (cell-free) TNF receptors; this may be a protective
mechanism which down-regulates the effects of TNF on host
cells.
The binding of TNF to its receptor may give rise to various
effects ranging from stimulation to apoptosis according to
the particular signalling pathway which is activated within the
target cell. Currently, these pathways (and the factors which
influence the choice of pathway) are incompletely understood,
but apoptosis seems to involve part of the cytoplasmic side
of the TNF receptor a region called the death domain.
Following TNFreceptor binding, the death domain appears to
associate with certain cytoplasmic factors including TRADD
(TNF receptor-associated death domain protein) and a serine
threonine kinase called RIP (receptor interacting protein); RIP
may activate caspase(s) such as IL-1b-converting enzyme (ICE)
(leading to APOPTOSIS) or it may phosphorylate (and inactivate)
the inhibitor IkB, thus activating the nuclear transcription factor
NF-kB.
tnpA gene See Tn3.
TnphoA See TRANSPOSON MUTAGENESIS.
tnpM gene See Tn21.
tnpR gene See Tn3.
toadstool Any umbrella-shaped basidiocarp, but particularly one
which is inedible or poisonous.
tobacco diseases For diseases of the tobacco plant see e.g.
GRANVILLE WILT, PERONOSPORA (blue mould), POTATO VIRUS Y
(e.g. veinal necrosis), TOBACCO MOSAIC VIRUS, TOBACCO NECROSIS
VIRUS and WILDFIRE DISEASE.
tobacco etch virus See POTYVIRUSES.
tobacco leafcurl virus See GEMINIVIRUSES.
tobacco mosaic virus (TMV) The type member of the TOBAMOVIRUSES. The TMV virion is a tubular filament (ca. 300
20 nm, central hole approx. 2 nm diam., S20
w ca. 194); it
comprises coat protein subunits (MWt ca. 17500) arranged in a
single right-handed helix with the ssRNA intercalated between
the turns of the helix (ca. three nucleotides per protein subunit).
780
TOL plasmid
infected fetus. Arthropod vectors (which remain infected for
life) are apparently unharmed. The Togaviridae contains four
genera (members of a genus being serologically related to
each other but unrelated to those of other genera): ALPHAVIRUS,
ARTERIVIRUS, PESTIVIRUS and RUBIVIRUS; possible members of
the family include LACTATE DEHYDROGENASE VIRUS and carrot
mottle virus. [Taxonomy: Intervirol. (1985) 24 125139.] (cf.
FLAVIVIRIDAE.)
The togavirus virion is spherical (ca. 5070 nm diam.) and
consists of a nucleocapsid (ca. 2835 nm diam.) which is
icosahedral in at least some species surrounded by a lipoprotein envelope. The nucleocapsid is composed of a single type
of core protein (C protein) associated with the RNA genome.
The envelope bears surface projections (spikes) composed of
two major glycoproteins, E1 and E2; in Semliki Forest virus a
third glycoprotein, E3, is associated with the spikes, but in other
alphaviruses E3 is released into the culture fluid in infected cell
cultures. The nature of the glycosylation of these proteins is
variable, depending at least in part on the nature of the host cell.
The envelope glycoproteins are responsible for haemagglutinating activity and for virus infectivity. [Structure of alphaviruses:
see e.g. Cell (2001) 105 58.]
The virus genome consists of a single molecule of linear
positive-sense ssRNA (MWt ca. 4 106 ); in those viruses which
have been investigated, the RNA is capped and polyadenylated. In alphaviruses, at least, the gene sequence is 5 nsP1nsP2nsP3nsP4CE3E2E1-3 , where nsP1nsP4
are non-structural proteins (apparently RNA-dependent RNA
polymerase components). [Nucleotide sequence of Sindbis virus:
Virol. (1984) 133 92110.]
Togavirus replication occurs in the host cell cytoplasm; the
process has been studied chiefly in the alphaviruses Semliki
Forest virus and Sindbis virus. In these viruses, the nonstructural proteins are synthesized directly from the (42S)
genome-length (+)-strand RNA, while structural proteins are
translated from capped and polyadenylated 26S subgenomic
RNA which is initiated internally on a full-length ()-strand
template. (Rubella virus employs a similar strategy, producing
40S genome-length and 24S subgenomic RNAs [JV (1984) 49
403408].) Translation is initiated at a single site, and the
proteins are generally cleaved from the nascent polyprotein
during translation. The synthesis of each type of viral RNA
(full-length ()-strand, full-length (+)-strand, and subgenomic)
is apparently regulated independently; 26S RNA is produced in
excess of 42S RNA, and genomic RNA is rapidly encapsidated,
so that a large excess of structural over non-structural proteins is
achieved. Virus maturation involves budding through the plasma
membrane or through intracytoplasmic membranes. [Overview
of the replication cycle: Book ref. 148, pp. 10211032.]
Many alphaviruses induce rapid and dramatic CPE in vertebrate cells (cf. RUBIVIRUS); host cell RNA and protein synthesis is rapidly arrested, and the cells eventually lyse. Some
alphaviruses can establish persistent infections in vertebrate
cells. [Effects of alphavirus infection on vertebrate cells: Book
ref. 150, pp. 465499.] Invertebrate cells are generally infected
persistently with no apparent adverse effects.
togaviruses Viruses of the TOGAVIRIDAE.
Tokophrya See SUCTORIA.
TOL plasmid An IncP-9 Pseudomonas PLASMID (ca. 117 kb)
which encodes the capacity to metabolize toluene and xylene.
(cf. CAM PLASMID; OCT PLASMID; SAL PLASMID.) [Degradative
plasmids of Pseudomonas: Book ref. 198, pp. 295323.]
TOL encodes the enzymes of a two-stage catabolic pathway
for the mineralization of toluene and xylene. Initially, these
TolA protein
tomato top necrosis virus See NEPOVIRUSES.
tomato yellow dwarf virus See GEMINIVIRUSES.
tomato yellow leafcurl virus See GEMINIVIRUSES.
tomato yellow mosaic virus See GEMINIVIRUSES.
tomato yellow net virus See LUTEOVIRUSES.
tomato yellow top virus See LUTEOVIRUSES.
tomaymycin See ANTHRAMYCIN.
tombusviruses (tomato bushy stunt virus group) A group of
ssRNA-containing PLANT VIRUSES which can infect a wide
range of angiosperms. Transmission occurs mechanically and
possibly via the soil. Type member: tomato bushy stunt virus
(TBSV); other members: e.g. artichoke mottled crinkle virus,
carnation Italian ringspot virus, Cymbidium ringspot virus, and
eggplant mottled crinkle virus. (Other possible members e.g.
carnation mottle virus, saguaro cactus virus, and turnip crinkle
virus appear on the basis of subgenomic dsRNA analysis
to have a different genome organization and may constitute
a separate group [Book ref. 80, pp. 8083].) [Serological
relationships among tombusviruses: JGV (1986) 67 7582.]
Virion: icosahedral, 30 nm diam., containing one molecule of
linear positive-sense ssRNA (MWt ca. 1.5 106 ). The capsid is
composed primarily of 180 molecules of a major coat protein.
Each coat protein molecule (386 amino acid residues) is folded
into three distinct domains (P, S and R): the S domains
form the tightly bonded icosahedral shell, the P domains form
surface projections, and the (N-terminal) R domains apparently
project inwards and may bind the genomic RNA; the P and
S domains are linked via a flexible hinge region. [Virion
structure: Book ref. 81, pp. 4350.] Within infected plant cells,
the virus particles occur in the cytoplasm and nucleus (often
associated with the nucleolus), sometimes forming crystalline
arrays; compact membranous inclusion bodies (multivesicular
bodies) occur in the cytoplasm.
tomentose Downy; woolly.
tomentum (lichenol.) A downy or felted mat of hyphae which
occurs (usually) on the lower surface of the thallus in certain
foliose lichens.
tomite A typically small, motile, non-feeding stage in the life
cycles of certain protozoa; it is generally formed, within a
CYST, by the division of a cell called a tomont. In e.g.
ICHTHYOPHTHIRIUS the tomite acts as a THERONT. In members of
the Apostomatida the tomite itself eventually encysts at a site on
a suitable host (becoming a phoront) and subsequently develops
into a cell capable of feeding (a trophont) which later develops
into a tomont; in some apostomes a stage known as a protomite
occurs between the tomont and tomite stages.
tomont See TOMITE.
TonA protein (FhuA protein) In Escherichia coli: an OUTER
MEMBRANE protein encoded by the tonA gene; it acts as a
receptor for e.g. colicin M and bacteriophages T1 and f80, and
is involved in the uptake of albomycin and ferrichrome.
TonB protein In e.g. Escherichia coli, a periplasmic protein
that shuttles between the cytoplasmic membrane and outer
membrane [Mol. Microbiol. (2003) 49 869882], supplying
energy (from pmf) to the outer membrane for the uptake of
e.g. ferric ironchelate complexes (see SIDEROPHORES); it is also
involved e.g. in the uptake of VITAMIN B12 by BINDING PROTEINDEPENDENT TRANSPORT.
The uptake of vitamin B12 across the outer membrane in
E. coli is pmf-dependent [JB (1993) 175 31463150]; it appears
that maximum activity of this (and other) TonB-dependent
systems requires the products of exbB and exbD (proteins in the
cytoplasmic membrane) which may stabilize TonB. ExbB and
II ,
(topo
an enzyme from E. coli which contains gyrase subunit A and a part of gyrase subunit B). The T4 enzyme and
topo II have been reported to relax positively or negatively
supercoiled DNA. In vitro, type II topoisomerases can form and
resolve catenanes and can also form and resolve knots. In a
model for the mechanism of type II topoisomerases, binding of
the enzyme initially introduces a sharp bend in the DNA, the
enzyme adopting a specific orientation with respect to the bend
and subsequently promoting unidirectional passage of the strands
through the break [PNAS (2001) 98 30453049].
Topoisomerase IV is a type II enzyme encoded by genes
parC and parE in E. coli. This enzyme can e.g. relax more
fully those negatively supercoiled molecules of DNA which
have been partially relaxed by topo I; topo IV appears to be
responsible solely for decatenation and for the resolution of
knots in E. coli [GD (2001) 15 748761].
topological winding number See DNA.
topotaxis A behavioural response in which a motile organism
moves (directly or indirectly) towards or away from a directional
stimulus. (cf. PHOBIC RESPONSE.)
Torbal jar See MCINTOSH AND FILDES ANAEROBIC JAR.
TORCH diseases A group of diseases comprising TOXOPLASMOSIS, RUBELLA, CYTOMEGALIC INCLUSION DISEASE, and HERPES
SIMPLEX each of which can cause abortion, stillbirth, severe
neonatal disease, and sometimes fetal tissue damage with consequent developmental abnormalities.
toroidal DNA See DNA TOROID.
Toroviridae A family of enveloped RNA viruses proposed to
include the BERNE VIRUS and serologically related viruses: e.g.
BREDA VIRUS and some human gastroenteritis viruses.
torr See PASCAL.
Torula A genus of fungi of the HYPHOMYCETES. T. herbarum is
common e.g. on dead grasses forming dark, velvety colonies,
and dark conidia in chains.
torula yeast A food yeast, Candida utilis (= Torulopsis utilis),
grown e.g. on ethanol or sulphite liquor waste (see SINGLE-CELL
PROTEIN); the yeast is pasteurized and dried before use. It is a
rich source of protein and vitamins and is used medicinally and
as a food additive.
torularhodin See CAROTENOIDS.
Torulaspora A genus of yeasts (family SACCHAROMYCETACEAE)
in which the cells are globose or ellipsoidal; vegetative reproduction occurs by multilateral budding. Pseudomycelium is not
formed. Vegetative cells are predominantly haploid (cf. SACCHAROMYCES). Ascus formation is preceded by conjugation usually
between a cell and its bud, but sometimes between independent cells; asci are persistent. Ascospores: globose or ellipsoidal, smooth- or rough-surfaced, 14 per ascus. Glucose and
certain other sugars are fermented vigorously; NO3 is not
assimilated. Species: T. delbrueckii (anamorph: Candida colliculosa), T. globosa (formerly e.g. Saccharomyces kloeckerianus),
and T. pretoriensis (formerly e.g. Saccharomyces pretoriensis);
strains have been isolated from fruit juice, wines, fermenting
cucumber brines, soil, faeces, etc. [Book ref. 100, pp. 434439.]
Torulopsis
A genus of yeasts (class HYPHOMYCETES), now
generally included within the genus CANDIDA [Book ref. 100,
p. 841]. Hyphae and pseudohyphae are generally not formed.
torulopsosis A MYCOSIS, now regarded as a form of CANDIDIASIS,
caused by Candida glabrata (= Torulopsis glabrata). The disease
(in man) is usually systemic, involving lungs, kidney, heart,
CNS etc.
torulosis Syn. CRYPTOCOCCOSIS.
total cell count See COUNTING METHODS.
783
Totiviridae
of pathogenesis. In many cases there is insufficient information
on the role of a given agent in pathogenesis to decide whether
or not it conforms to the above definition.
In some cases the known activity of a toxin is sufficient to
accoun