- Volume 134, Issue 3, 1988
Volume 134, Issue 3, 1988
- Pathogenicity And Medical Microbiology
-
-
-
Lipopolysaccharide Masking of Gonococcal Outer-membrane Proteins Modulates Binding of Bactericidal Cathepsin G to Gonococci
More LessHuman polymorphonuclear leucocyte (PMN) lysosomal cathepsin G exerts potent bactericidal action against Neisseria gonorrhoeae in vitro, independent of its serine esterase activity. The results presented demonstrate that (1) bactericidal, diisopropylfluorophosphate-treated cathepsin G binds in a specific and saturable manner to the surface of gonococci, (2) loss of carbohydrates in gonococcal LPS due to mutation increases total and specific binding of cathepsin G, and (3) at least three outer-membrane proteins (OMPs) (PIA, PIII. and a 45 kDa OMP) interact with cathepsin G. Taken together, the results suggest that gonococcal susceptibility to the lethal action of cathepsin G, and perhaps susceptibility of gonococci to oxygen-independent killing by PMNs, is controlled by LPS-masking of cathepsin-G-binding OMPs.
-
-
-
-
DNA Hybridization with Hardjobovis-specific Recombinant Probes as a Method for Type Discrimination of Leptospira interrogans Serovar hardjo
More LessRestriction endonuclease analysis of DNA of Leptospira interrogans, serovar hardjo, showed two distinct types within this serovar. These two types, hardjoprajitno and hardjobovis, cannot be differentiated by monoclonal antibodies. Application of 32P- or biotin-labelled total DNA probes in dot-blot or in situ hybridization assays showed a high sensitivity of the assays but also considerable cross-hybridization. Therefore, a genomic library of hardjobovis was constructed and a number of hardjobovis-specific recombinant clones were isolated. Finally, four clones were selected on the basis of a strong hybridization signal and a high specificity for hardjobovis as compared to hardjoprajitno. In a dot-blot assay as well as in in situ hybridization experiments all four clones gave strong signals, and no cross-hybridization with hardjoprajitno was observed in either type of assay. Our results indicate that specific recombinant DNA probes might provide tools for routine diagnosis and classification in cases of hardjo infections.
-
-
-
Nucleotide Sequence of the Pilin Gene of Bacteroides nodosus 340 (Serogroup D) and Implications for the Relatedness of Serogroups
More LessThe gene encoding pilin of Bacteroides nodosus 340 has been isolated and the nucleotide sequence determined. The gene is present as a single copy within the B. nodosus genome and a protein of M r 16683 can be predicted from the proposed coding region. A comparison of the predicted amino acid sequence with pilin from other strains of B. nodosus indicated that the protein of strain 340 (serogroup D) has a high degree of similarity with pilin of strain 265 (serogroup H). The degree of similarity between pilins from these strains and from other B. nodosus serogroups is no greater than that between B. nodosus pilins and the homologous proteins of several different bacterial species. These findings suggest that serogroups D and H may form a subset of B. nodosus serogroups.
-
-
-
Effect of Dilution Rate and Mg2+ Limitation on Toxic Shock Syndrome Toxin-1 Production by Staphylococcus aureus Grown in Defined Continuous Culture
More LessA toxic shock syndrome isolate of Staphylococcus aureus was grown in a chemostat, in a defined synthetic medium of six amino acids, glucose, two vitamins and salts. Steady states were achieved under limiting and replete Mg2+ conditions and at a range of relative specific growth rates. The biomass and toxic shock syndrome toxin-1 (TSST-1) were estimated at each condition. Under Mg2- limitation the biomass and TSST-1 production rates were reduced compared to Mg2+ replete conditions. Optimal TSST-1 production occurred at 0.81 relative specific growth rate.
-
-
-
Vero Cytotoxin Production and Presence of VT Genes in Escherichia coli Strains of Animal Origin
More LessVero cytotoxin (VT) production has been studied in 34 Escherichia coli strains isolated from animals with enteric diseases. The strains were tested by DNA hybridization with probes for VT1 and VT2 sequences and also in toxin neutralization experiments with specific antisera. Twenty bovine strains, belonging to nine different O serogroups, produced VT1 or VT2 but not both toxins. In contrast, all 14 porcine strains of four different O serogroups produced VT2 only. Six of these porcine strains, belonging to serogroups 0138, 0139 and 0141, were isolated from cases of oedema disease. In general, the porcine isolates produced toxin at a lower level than the bovine strains.
-
-
-
Molecular Cloning of the Shv-1 β-Lactamase Gene and Construction of an Shv-1 Hybridization Probe
More LessWe have cloned the Shv-1 β-lactamase gene from the R1010 plasmid into pACYC184. By subcloning and transposon mutagenesis we have localized the gene to a 1·6 kb BscI-SalI fragment of R1010, which is present in the recombinant plasmid pUB8. A 900 bp PstI fragment of pUB8 was shown to be a specific hybridization probe by testing against plasmids which encode 17 different β-lactamase enzymes. A comparison was made of the sensitivity of the Shv-1 probe labelled with either [35S]dCTP or with photobiotin.
-
- Physiology And Growth
-
-
-
The Role of Glycerol in Osmotolerance of the Yeast Debaryomyces hansenii
More LessTransfer of growing cells of the salt-tolerant yeast Debaryomyces hansenii to media of higher salinity resulted in an increased production and intracellular accumulation of glycerol, which was proportional to the magnitude of the shift in salinity. Stress solutes other than NaCl, when added in iso-osmolar concentrations, promoted the accumulation of similar amounts of glycerol. Cells grown at high salinity rapidly lost glycerol when returned to media of lower salinity and the loss was greater when the cells were transferred to more dilute media. A mutant strain of D. hansenii showed poor glycerol production and was inhibited by NaCl at concentrations about half the maximum tolerated by the wild-type. Growth of this mutant occurred at otherwise inhibitory NaCl concentrations if the medium was supplemented with a low concentration of glycerol. The added glycerol was intracellularly accumulated to levels that increased with salinity and were only slightly lower than the corresponding wild-type levels. Glycerol additions above the growth promoting level had little effect on growth rate but caused substantial shortening of the lag phase. Osmoprotectants other than glycerol did not permit growth to occur. The mutant was isolated as a glycerol non-utilizer but displayed growth in glycerol media at increased NaCl concentrations.
-
-
-
-
Extraordinarily Rapid Appearance of a β-Fructofuranosidase (Exo-inulase)-hyperproducing Mutant in Continuous Culture of Kluyveromyces fragilis
More LessA wild-type strain of the yeast Kluyveromyces fragilis was grown in continuous culture on inulin-, fructose- and glucose-limited media. In the presence of organic nitrogen, all three carbon sources supported an extremely rapid changeover to a homogeneous mutant cell population that exhibited hyperproduction of β-fructofuranosidase (exo-inulase). The non-specific role of the carbon substrate in the takeover suggested co-regulation of inulase synthesis and early glycolytic pathway enzymes such as hexokinase, resulting in gratuitous hyperproduction of inulase. The rate of mutant appearance increased linearly with a decrease in dilution rate as well as carbon/nitrogen ratio, implying that the responsible forces were related to the residual concentration of the limiting carbon substrate. Under optimum conditions, mutant cells were detected within only 40 h (2·9 generations) from the start of continuous culture, at least 6·5 times faster than predicted. The maximum rate of displacement was as high as 54% per generation, or more than 12 times greater than predicted from the differential growth rate between the wild-type and mutant strain. These extraordinarily rapid takeovers point to a very fast and ongoing genetic change triggered by growth under severe stress.
-
-
-
Mycobactins and Exochelins of Mycobacterium tuberculosis, M. bovis, M. africanum and Other Related Species
More LessFollowing iron-deficient growth, mycobactins and exochelins were isolated from 11 strains of Mycobacterium tuberculosis (including type strains of the virulent H37Rv and avirulent H37Ra organisms) as well as from M. bovis (one strain), M. bovis BCG (two strains), M. africanum (eight strains) and M. xenopi (one strain) but not from M. microti (one strain). The mycobactins from the tuberculosis group (M. tuberculosis, M. bovis and M. africanum) were identical and could each be resolved into four compounds by thin-layer chromatography (TLC) and into several fractions by high-performance liquid chromatography, supporting previous claims that this group is a single taxon. Exochelins were all chloroform-soluble and showed no species specificity; no single exochelin was recognized by TLC that had not been previously seen in M. avium or a related species.
-
-
-
Continued Growth of Escherichia coli after Stopping Medium Addition to a K+-limited Chemostat Culture
More LessThe steady-state bacterial dry wt of Escherichia coli, growing under K+-limited conditions in the chemostat, was inversely dependent on the growth rate. This phenomenon was more carefully investigated in medium-flow stop experiments. Growth did not stop immediately but continued for a time, initially at the same rate as before. The dry wt increased to a value corresponding to a steady-state growth rate near zero, independent of the initial specific growth rate. This was observed in both the wild-type strain and a mutant that lacked the high-affinity K+ uptake system. The wild-type strain maintained a low extracellular K+ concentration both in the chemostat under steady-state conditions and after stopping the medium flow. The mutant, on the other hand, maintained a much higher extracellular K+ concentration in the steady state, which decreased to much lower values after stopping the medium flow. From the increase in bacterial dry wt and the low external K+ concentration after stopping the medium flow it is concluded that the intracellular K+ is redistributed among the cells, including new cells. The growth yield on K+ was highest in the stationary growth phase of a batch culture and all steady-state cultures converged ultimately to this yield value after the medium flow had been stopped. It is proposed that the growth rate of E. coli under K+-limited conditions is determined by the intracellular K+ concentration.
-
-
-
Regulation of Trehalase Activity during the Cell Cycle of Saccharomyces cerevisiae
More LessSynchronous cultures of Saccharomyces cerevisiae prepared by selection of small unbudded cells from an elutriating rotor were used to measure trehalase activity during the cell cycle. After the small cells had been removed from the rotor, the remainder was used to prepare asynchronous control cultures. Both synchronous and control cultures were studied for two cell cycles. In asynchronous cultures the trehalase activity of crude cell lysates rose continuously. In synchronized populations trehalase activity increased from the beginning of budding onwards. However, around the period of cell division the enzyme activity dropped rapidly but transiently by more than 5-fold. The same changes were found during the second budding cycle. Measurements of invertase and glucose-6-phosphate dehydrogenase activities in the same synchronous and asynchronous cultures revealed a continuous increase for both enzymes. Incubation of cell lysates with cAMP-dependent protein kinase before assaying for trehalase resulted in a 2-fold enhancement of enzyme activity in asynchronous control cultures. In synchronized cells this treatment also led to a significant stimulation of trehalase activity, and largely abolished the cell-cycle-dependent oscillatory pattern of enzyme activity. These results suggest that the activity of trehalase during the cell cycle is regulated, presumably at the post-translational level, by a phosphorylation-dephosphorylation mechanism.
-
-
-
Presence of Anaplerotic Reactions and Transamination, and the Absence of the Tricarboxylic Acid Cycle in Mollicutes
More LessCell extracts of the fermentative Mollicutes Acholeplasma laidlawii B-PG9, Acholeplasma morum S2, Mycoplasma capricolum 14, Mycoplasma gallisepticum S6, Mycoplasma pneumoniae FH, Mycoplasma hyopneumoniae J and M. genitalium G-37, and the non-fermentative Mycoplasma hominis PG-21, Mycoplasma hominis 1620 and Mycoplasma bovigenitalium PG-11 were examined for 39 cytoplasmic enzyme activities associated with the tricarboxylic acid (TCA) cycle, transamination, anaplerotic reactions and other enzyme activities at the pyruvate locus. Malate dehydrogenase (EC 4.2.1.2) was the only TCA-cycle-associated enzyme activity detected and it was found only in the eight Mycoplasma species. Aspartate aminotransferase (EC 2.6.1.1) activity was detected in all Mollicutes tested except M. gallisepticum S6. Malate synthetase (EC 4.1.3.2) activity, in the direction of malate formation, was found in the eight Mycoplasma species, but not in any of the Acholeplasma species. Phosphoenolpyruvate (PEP) carboxylase (EC 4.1.1.31) was detected in the direction of oxaloacetate (OAA) formation in both Acholeplasma species, but not in any of the Mycoplasma species. Pyruvate carboxylase (EC 6.4.1.1), pyruvate kinase (EC 2.7.1.40), pyruvate dehydrogenase (EC 1.2.4.1) and lactate dehydrogenase (EC 1.1.1.27) activities were found in all ten Mollicutes tested. No activities were detected in any of the ten Mollicutes for aspartase (EC 4.3.1.1), malic enzyme (EC 1.1.1.40), PEP carboxytransphosphorylase (EC 4.1.1.38), PEP carboxykinase (EC 4.1.1.32) or pyruvate orthophosphate dikinase (EC 2.7.9.1). In these TCA-cycle-deficient Mollicutes the pyruvate-OAA locus may be a point of linkage for the carbons of glycolysis, lipid synthesis, nucleic acid synthesis and certain amino acids. CO2 fixation appears obligatory in the Acholeplasma species and either CO2 fixation or malate synthesis appears obligatory in the Mycoplasma species.
-
-
-
An Extracellular Blood-anticoagulant Glycopeptide Produced Exclusively during Vegetative Growth by Myxococcus xanthus and Other Myxobacteria Is Not Co-regulated with Other Extracellular Macromolecules
More LessWe have shown that the blood anticoagulant activity (BAA) secreted by Myxococcus xanthus (designated myxaline) is a heat-stable molecule: a high-molecular-mass extracellular fraction also with an apparent BAA is a thermolabile protease. This property allowed us to assay the BAA content in crude boiled culture supernatants and to study the conditions under which it is produced. Heat-stable BAA is strictly extracellular and its production is restricted to vegetative growth in M. xanthus. Unlike the other extracellular proteins, its production is not affected by mutations that regulate secretion; mutations that modify the extracellular proteolytic activity do not modulate the amount of myxaline produced either. Several other species of Myxococcus and one other myxobacterial species produce a heat-stable BAA during vegetative growth.
-
- Systematics
-
-
-
Taxonomic Study of Non-alkaliphilic Halococci
More LessNinety-six extremely halophilic, non-alkaliphilic cocci were isolated from several salterns in different geographical areas of Spain. These strains, together with seven reference strains of the genus Halococcus, were characterized by means of 114 phenotypic features, the results being analysed by numerical techniques using the simple matching (SSM ) coefficient and the unweighted pair group clustering (UPGMA) algorithm. At the 70% similarity level, four phenons were obtained. Phenon A contained 87 strains, including all the reference strains, and was considered to comprise members of the only named species of the genus Halococcus, H. morrhuae. Phenons B and C, which included five and seven strains respectively, showed greater metabolic versatility than phenon A. The four strains belonging to phenon D were significantly different from the other phenons in that they produced acid from glucose and were able to use most of the organic compounds tested. The results indicate that there is phenotypic diversity among the members of the genus Halococcus and that phenon D may constitute a new taxon.
-
-
-
-
Numerical Taxonomy of Moderately Halophilic Gram-negative Rods from an Inland Saltern
A total of 174 moderately halophilic bacteria was isolated from an inland saltern with athalassohaline characteristics, located in La Malá, Granada, Spain. The results of 118 phenotypic tests were submitted to a numerical analysis with ten reference strains using simple matching (SSM ) and Jaccard (SJ ) coefficients. Clustering was done by the unweighted pair-group method of association (UPGMA), single linkage and complete linkage analysis. Five phenons were found at the 67% similarity level (SSM ). Phenon A included 74 strains assigned to Vibrio; 22 bacteria belonging to phenon B were assigned to the genus Alteromonas; strains of phenon C were assigned to Deleya (43 strains) and Acinetobacter (7 strains); phenon D resembled Pseudomonas (13 strains); phenon E could be related to Flavobacterium oceanosedimentum (9 strains).
-
-
-
An Assessment of Taxonomic Congruence between DNA—DNA Hybridization and Pyrolysis Gas—Liquid Chromatographic Classifications
More LessThe existence of subgroups within Bacillus megaterium has been reported previously on the basis of DNA-DNA hybridization and DNA base composition studies. In this study the strains used to define these subgroups have been reanalysed by pyrolysis gas-liquid chromatography. The resultant two-group classification of the test strains was directly comparable with that obtained from the previous nucleic acid analyses at the between-group level. However, comparisons of the test strains at the within-group level proved less successful.
-
-
-
Biochemical and Physiological Characterization of Colony Form Variants in Xenorhabdus spp. (Enterobacteriaceae)
More LessPrimary and secondary form variants of Xenorhabdus isolated from 21 strains (13 species) of Steinernematidae and Heterorhabditidae were tested for 240 biochemical and physiological characters. Primary form variants, isolated from the infective stage nematodes, could always be distinguished from the secondary by adsorption of neutral red from MacConkey agar. Lecithinase, antibiotic activity and/or adsorption of bromothymol blue were useful for distinguishing the variants of most strains. The variants of all strains also differed for other characteristics but the distinguishing characteristics varied from strain to strain. The importance of including both variants of each strain and of using appropriate methods in the study of Xenorhabdus taxonomy was demonstrated.
-
Volumes and issues
-
Volume 170 (2024)
-
Volume 169 (2023)
-
Volume 168 (2022)
-
Volume 167 (2021)
-
Volume 166 (2020)
-
Volume 165 (2019)
-
Volume 164 (2018)
-
Volume 163 (2017)
-
Volume 162 (2016)
-
Volume 161 (2015)
-
Volume 160 (2014)
-
Volume 159 (2013)
-
Volume 158 (2012)
-
Volume 157 (2011)
-
Volume 156 (2010)
-
Volume 155 (2009)
-
Volume 154 (2008)
-
Volume 153 (2007)
-
Volume 152 (2006)
-
Volume 151 (2005)
-
Volume 150 (2004)
-
Volume 149 (2003)
-
Volume 148 (2002)
-
Volume 147 (2001)
-
Volume 146 (2000)
-
Volume 145 (1999)
-
Volume 144 (1998)
-
Volume 143 (1997)
-
Volume 142 (1996)
-
Volume 141 (1995)
-
Volume 140 (1994)
-
Volume 139 (1993)
-
Volume 138 (1992)
-
Volume 137 (1991)
-
Volume 136 (1990)
-
Volume 135 (1989)
-
Volume 134 (1988)
-
Volume 133 (1987)
-
Volume 132 (1986)
-
Volume 131 (1985)
-
Volume 130 (1984)
-
Volume 129 (1983)
-
Volume 128 (1982)
-
Volume 127 (1981)
-
Volume 126 (1981)
-
Volume 125 (1981)
-
Volume 124 (1981)
-
Volume 123 (1981)
-
Volume 122 (1981)
-
Volume 121 (1980)
-
Volume 120 (1980)
-
Volume 119 (1980)
-
Volume 118 (1980)
-
Volume 117 (1980)
-
Volume 116 (1980)
-
Volume 115 (1979)
-
Volume 114 (1979)
-
Volume 113 (1979)
-
Volume 112 (1979)
-
Volume 111 (1979)
-
Volume 110 (1979)
-
Volume 109 (1978)
-
Volume 108 (1978)
-
Volume 107 (1978)
-
Volume 106 (1978)
-
Volume 105 (1978)
-
Volume 104 (1978)
-
Volume 103 (1977)
-
Volume 102 (1977)
-
Volume 101 (1977)
-
Volume 100 (1977)
-
Volume 99 (1977)
-
Volume 98 (1977)
-
Volume 97 (1976)
-
Volume 96 (1976)
-
Volume 95 (1976)
-
Volume 94 (1976)
-
Volume 93 (1976)
-
Volume 92 (1976)
-
Volume 91 (1975)
-
Volume 90 (1975)
-
Volume 89 (1975)
-
Volume 88 (1975)
-
Volume 87 (1975)
-
Volume 86 (1975)
-
Volume 85 (1974)
-
Volume 84 (1974)
-
Volume 83 (1974)
-
Volume 82 (1974)
-
Volume 81 (1974)
-
Volume 80 (1974)
-
Volume 79 (1973)
-
Volume 78 (1973)
-
Volume 77 (1973)
-
Volume 76 (1973)
-
Volume 75 (1973)
-
Volume 74 (1973)
-
Volume 73 (1972)
-
Volume 72 (1972)
-
Volume 71 (1972)
-
Volume 70 (1972)
-
Volume 69 (1971)
-
Volume 68 (1971)
-
Volume 67 (1971)
-
Volume 66 (1971)
-
Volume 65 (1971)
-
Volume 64 (1970)
-
Volume 63 (1970)
-
Volume 62 (1970)
-
Volume 61 (1970)
-
Volume 60 (1970)
-
Volume 59 (1969)
-
Volume 58 (1969)
-
Volume 57 (1969)
-
Volume 56 (1969)
-
Volume 55 (1969)
-
Volume 54 (1968)
-
Volume 53 (1968)
-
Volume 52 (1968)
-
Volume 51 (1968)
-
Volume 50 (1968)
-
Volume 49 (1967)
-
Volume 48 (1967)
-
Volume 47 (1967)
-
Volume 46 (1967)
-
Volume 45 (1966)
-
Volume 44 (1966)
-
Volume 43 (1966)
-
Volume 42 (1966)
-
Volume 41 (1965)
-
Volume 40 (1965)
-
Volume 39 (1965)
-
Volume 38 (1965)
-
Volume 37 (1964)
-
Volume 36 (1964)
-
Volume 35 (1964)
-
Volume 34 (1964)
-
Volume 33 (1963)
-
Volume 32 (1963)
-
Volume 31 (1963)
-
Volume 30 (1963)
-
Volume 29 (1962)
-
Volume 28 (1962)
-
Volume 27 (1962)
-
Volume 26 (1961)
-
Volume 25 (1961)
-
Volume 24 (1961)
-
Volume 23 (1960)
-
Volume 22 (1960)
-
Volume 21 (1959)
-
Volume 20 (1959)
-
Volume 19 (1958)
-
Volume 18 (1958)
-
Volume 17 (1957)
-
Volume 16 (1957)
-
Volume 15 (1956)
-
Volume 14 (1956)
-
Volume 13 (1955)
-
Volume 12 (1955)
-
Volume 11 (1954)
-
Volume 10 (1954)
-
Volume 9 (1953)
-
Volume 8 (1953)
-
Volume 7 (1952)
-
Volume 6 (1952)
-
Volume 5 (1951)
-
Volume 4 (1950)
-
Volume 3 (1949)
-
Volume 2 (1948)
-
Volume 1 (1947)