- Volume 137, Issue 11, 1991
Volume 137, Issue 11, 1991
- Review Article
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- Biochemistry
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Purification, characterization and comparison of two non-haem bromoperoxidases from Streptomyces aureofaciens ATCC 10762
More LessTwo non-haem bromoperoxidases (BPO 1 and BPO 2) were purified from the 7-chlorotetracycline-producing strain Streptomyces aureofaciens ATCC 10762. Both enzymes showed azide-insensitive brominating activity, and bromide-dependent peroxidase activity. BPO 1 was a dimer (M r 65000) with subunits of identical size (M r 31000). The pI was estimated to be 4·5. The enzyme did not cross-react with antibodies raised against the non-haem bromoperoxidase (M r 90000) from S. aureofaciens Tü24, a strain that also produces 7-chlorotetracycline. The M r of BPO 2 was estimated to be 90000. The enzyme had three identical subunits (M r 31000), and its isoelectric point was 3·5, identical with that of the bromoperoxidase from S. aureofaciens Tü24. Moreover, BPO 2 was immunologically identical with the bromoperoxidase from S. aureofaciens Tü24, although both it and BPO 1 could be distinguished electrophoretically from the latter bromoperoxidase.
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Alkene monooxygenase from Mycobacterium: a multicomponent enzyme
More LessA NADH- or NADPH-dependent alkene monooxygenase (AMO) activity has been detected in cell-free extracts of the ethene-utilizing Mycobacterium E3 and Mycobacterium aurum L1. The activity was not linear with protein concentration in the assay suggesting AMO is a multicomponent enzyme. The inhibition pattern of AMO activity was very similar to the inhibition patterns published for the three-component soluble methane monooxygenases. Fractionation of crude extracts revealed that combination of two fractions was required to restore alkene monooxygenase activity. The first fraction was inhibited by acetylene, indicating it contained an oxygenase component. The second fraction contained reductase activity which was absent from non-induced cells. This reductase activity is probably the NADH-acceptor reductase of AMO.
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A membrane-bound pyrophosphatase from respiratory membranes of Rhodospirillum rubrum
More LessA pyrophosphatase activity was found in respiratory membranes of Rhodospirillum rubrum. This activity was specific for pyrophosphate and was inhibited by dicyclohexylcarbodiimide, NaF and pyrophosphate analogues, but not by oligomycin or LiCl. The divalent cation selectivity was Zn2+ > Mg2+ > Co2+ > Ca2+, and the pH dependence was the same as that of the membrane-bound pyrophosphatase of chromatophores (optimum pH 6·5). The pyrophosphate hydrolysis activity of respiratory membranes was inhibited by 1-butanol. The enzyme was solubilized by Triton X-100, and the activity of the solubilized enzyme was stimulated by phospholipids. The respiratory-membrane enzyme ran in native electrophoresis with the same R F as the membrane-bound pyrophosphatase of chromatophores. Antibodies raised against both enzymes cross-reacted with each other. These findings show that a membrane-bound pyrophosphatase is present in respiratory membranes of R. rubrum and is similar to the enzyme of photosynthetic membranes.
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Identification of a sterol mutant of Neurospora crassa deficient in Δ14,15-reductase activity
More LessSummary: A mutant (erg-3) of Neurospora crassa resistant to the polyene antibiotic nystatin was compared with its sensitive, wild-type parent to detect differences in sterol composition using gas chromatography—mass spectrometry. The major sterol in wild-type mycelia, comprising 80% of the total, was ergosterol. The major sterols in mutant mycelia, comprising 86% of the total, were δ814-sterols. It is proposed that the nystatin-resistant strain is unable to synthesize ergosterol because it lacks δ1415-reductase activity as a result of a mutation in the erg-3 gene.
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Long-chain chloroalkane utilization by a marine protozoan
Summary: A long-chain chloroalkane, 1-chlorooctadecane, was biotransformed by a marine amoeba, Trichosphaerium 1–7, and utilized by this organism as a carbon source. Haloalkane metabolism was accompanied by marked cell darkening which may represent xenobiotic-induced melanin biosynthesis. Radiolabelled carbon atoms derived from 1-chloro[1-14C]octadecane were incorporated into cellular proteins and organic intermediates, including fatty acids. Gas chromatography and mass spectrometry analyses of the fatty acid methyl ester derivatives, however, showed that they were not chlorinated. [1-14C]Octadecanoic acid methyl ester was detected by mass spectrometry, but hexadecanoic acid methyl ester did not contain detectable 14C. These data suggest that the amoebae convert the chloroalkane to the corresponding fatty acid by oxidative dehalogenation.
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- Ecology
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Measurement of the force necessary for removal of bacterial cells from a quartz plate
More LessSummary: The force necessary to remove the cells of a bacterium, an isolate (Bacillus sp.) from grassland soil, from a quartz plate was investigated in phosphate buffer solution by using a well-defined liquid flow caused by electroosmosis. The cells were not removed at a specific strength of removal force but removed over a wide range of force, about 10−14-10−12 N per cell. An exponential relation was observed between the removal force and the number of removed cells in media of pH 7·0,80 and 9·0; more cells were removed by a smaller force. Experiments in media of different pH values in the range 3·0 to 9·0 showed that greater force was necessary to remove the cells in media of lower pH. The smaller electrostatic repulsion between the bacterial cells and the quartz plate at lower pH values was considered to result in the greater force needed for removal. The relation between the strength of the removal force and the strength of the adhesion force of the bacterial cells was considered. The findings showed that the cell adhesion was reversible and that the adhesion site was located near the end of the cell.
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- Genetics And Molecular Biology
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The aconitase of Escherichia coli: purification of the enzyme and molecular cloning and map location of the gene (acn)
More LessThe aconitase of Escherichia coli was purified to homogeneity, albeit in low yield (0·6%). It was shown to be a monomeric protein of M r 95000 or 97500 by gel filtration and SDS-PAGE analysis, respectively. The N-terminal amino acid sequence resembled that of the Bacillus subtilis enzyme (citB product), but the similarity at the DNA level was insufficient to allow detection of the E. coli acn gene using a 456 bp citB probe. Phages containing the acn gene were isolated from a λ-E. coli gene bank by immunoscreening with an antiserum raised against purified bacterial enzyme. The acn gene was located at 28 min (1350 kb) in the physical map of the E. coli chromosome by probing Southern blots with a fragment of the gene. Attempts to locate the gene using the same procedure with oligonucleotide probes encoding segments of the N-terminal amino acid sequence were complicated by the lack of probe specificity and an inaccuracy in the physical map of Kohara et al. (Cell 50, 495–508, 1987). Aconitase specific activity was amplified some 20-200-fold in cultures transformed with pGS447, a derivative of pUC119 containing the acn gene, and an apparent four-fold activation—deactivation of the phagemid-encoded enzyme was observed in late exponential phase. The aconitase antiserum cross-reacted with both the porcine and Salmonella typhimurium (M r 120000) enzymes.
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Characterization of the 5′ flanking region of the Escherichia coli ppa gene encoding inorganic pyrophosphatase: mutations in the ribosome-binding site decrease the level of ppa mRNA
We have previously cloned and sequenced the ppa gene, encoding inorganic pyrophosphatase (PPase), of Escherichia coli K12 [Lahti, R., Pitkäranta, T., Valve, E., Ilta, I., Kukko-Kalske, E. & Heinonen, J. (1988) Journal of Bacteriology 170, 5901–5907]. In this work mutations were constructed in the 5′ flanking region of E. coli ppa and the effect on expression was determined. The minimum length of the fully active ppa 5′ flanking region was shown to be 117 bp. Further deletion decreased the activity, and upon deletion to nucleotide –37 the promoter activity was totally lost. A clear point of inflection was observed in the inactivation upon deletion over the nucleotide –50. This is consistent with the fact that by binding to promoters RNA polymerase holoenzyme generally covers the –50 to +20 region in E. coli genes. When the –35 sequence of ppa, AAGACA, was mutated to AAAACA, ppa expression, as measured by PPase production, decreased to 20% of the wild-type, whereas by the change of the –10 sequence, TATAAT, to TTTAAT or TATAAA, the ppa gene was totally inactivated. Furthermore, when the ribosome-binding site (RBS) sequence, AGGAAA, was altered to AAGAAA, PPase production decreased to 19% of the wild-type. Surprisingly, when the RBS sequence was mutated to the consensus RBS sequence, AGGAGG, the intracellular levels of both ppa mRNA and PPase decreased drastically. The implications of these results are discussed.
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Electrophoretic karyotypes of clinically isolated yeasts of Candida albicans and C. glabrata
More LessOne-hundred-and-four isolates of yeast were collected from the vaginas of 97 outpatients. The isolates were identified by their characteristics in a carbohydrate assimilation test, a serological test and from their morphology. Candida albicans and Candida glabrata were the major isolates (75% and 20%, respectively). The karyotypes of the isolates were analysed by pulsed-field gel electrophoresis and almost all the karyotypes were distinguishable from one another when the band mobilities were carefully compared. Characteristics and karyotypes were not directly correlated, but seven C. albicans isolates (from six patients) had a common atypical karyotype and shared the same phenotype. These isolates are inferred to be generated by a wide genomic reorganization and mutation and the phenotypic changes may be advantageous for survival. The karyotypes of the isolates recovered from individual patients after intervals of 1–6 months were all identical except for one or two highly variable bands which were identified with an rDNA probe. This suggests that the variable bands are too variable to be useful for distinguishing strains, but from the patterns of the identical bands (i.e. except for the variable bands) we concluded that strains from individual patients do not change, at least over short periods. This, coupled with the extensive inter-isolate variability in karyotype, will be useful for Candida source determination and epidemiological studies.
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Nucleotide sequence of a Lactococcus lactis gene cluster encoding adenylate kinase, initiation factor 1 and ribosomal proteins
More LessSummary: We have previously isolated a putative promoter from the Lactococcus lactis subsp. lactis chromosome. We now report the sequence of the promoter fragment and its extension in the 5′-direction. The region contains several open-reading frames which correspond to ribosomal protein L15, SecY, adenylate kinase, initiation factor 1 and ribosomal proteins B and S13. The order of the genes, rplO (L15), secY, adk, infA, rpmJ (B) and rpsM (S13), is similar to that in the spc and α operon region of Bacillus subtilis, with the exception of the map gene, coding for methionine amino peptidase, which is located between adk and infA in B. subtilis. The putative promoter is located between adk and infA.
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The possible involvement of protein synthesis in the injection of PL-1 phage genome into its host, Lactobacillus casei
More LessThe process of genome DNA injection, after adsorption, by phage PL-1 into host cells of Lactobacillus casei was monitored by using the electron microscope. Injection of DNA was inhibited by the protein-synthesis inhibitors chloramphenicol and erythromycin at concentrations where the colony-forming ability of cells not infected by phage was unaffected. The results suggest that protein synthesis may be involved in some way in the process of genome injection.
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- Pathogenicity And Medical Microbiology
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Restriction pattern of the major outer-membrane protein gene provides evidence for a homogeneous invasive group among ruminant isolates of Chlamydia psittaci
More LessThirty-six ruminant isolates of Chlamydia psittaci, previously classified as invasive or non-invasive in a mouse model of virulence, were compared by analysing AluI restriction patterns of the major outer-membrane protein (MOMP) gene after DNA amplification by the polymerase chain reaction. The 24 invasive isolates, although from various origins, all belonged to serotype 1 and represented a strictly homogeneous group sharing a specific MOMP-gene restriction pattern that was not observed in the non-invasive strains. On the other hand, the 12 non-invasive strains, although all belonging to serotype 2, constituted a heterogeneous group with eight distinct MOMP-gene restriction patterns. However, all eight patterns shared a 180 bp fragment or the corresponding restricted fragments of 110 and 70 bp. MOMP-gene restriction patterns also clearly distinguished the ruminant strains from an avian C. psittaci isolate, a C. pneumoniae isolate and two C. trachomatis isolates which were studied for comparison. The homogeneous character of the invasive C. psittaci strains argues strongly for their genetic relatedness. Our results illustrate the usefulness of the MOMP-gene restriction mapping in typing chlamydiae.
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Variation in the expression of cell envelope proteins of coagulase-negative staphylococci cultured under iron-restricted conditions in human peritoneal dialysate
Summary: Strains of coagulase-negative staphylococci (CNS), including Staphylococcus epidermidis, S. hominis, S. warnerii, S. simulans, S. capitis, S. haemolyticus and S. saprophyticus, were isolated from patients with continuousambulatory-peritoneal-dialysis-related peritonitis. The cell wall and cytoplasmic membrane protein profiles of CNS strains cultured in either nutrient broth (NB) or pooled human peritoneal dialysate (HPD) were compared. Some interspecies variation in both the wall and membrane protein profiles was noted. However, the cell wall protein profiles of HPD-grown CNS strains differed markedly from those cultured in NB. Growth in HPD resulted in a marked reduction in the total number of cell-wall-associated proteins but up to three antigenically related proteins in the 40–56 kDa range, depending on the species, predominated. Growth in HPD also resulted in the induction of two iron-repressible cytoplasmic membrane proteins (IRMPs) of 32 and 36 kDa in S. epidermidis. Other CNS strains only appeared to express a single IRMP, which varied in molecular mass from 32 to 36 kDa. Whilst the IRMP in these CNS strains showed considerable antigenic homology with the 32 kDa IRMP, the S. warneri IRMP showed cross-reactivity with both the 32 and 36 kDa IRMPs of S. epidermidis. Immunoblotting experiments revealed that whilst the CNS cell wall proteins were poorly immunogenic, the IRMPs were the immunodominant CNS protein antigens, reacting strongly with antibodies present in HPD. This finding provides evidence to suggest that the IRMPs are expressed in vivo during infection.
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Capsulation gene loss and ‘rescue’ mutations during the Cap+ to cap- transition in Huemophilus influenzae type b
More LessSummary: Genes for Haemophilus influenzae type b capsule expression are duplicated to form a potentially unstable structure, cap, of directly-repeated chromosomal regions of approximately 17 kb. Capsule-deficient mutants arise in a two-stage process, initiated by rec-dependent reduction of this region from two copies to one. This recombinational event is usually lethal, only about 1/200 surviving to form slow-growing colonies of organisms that continue to synthesize polysaccharide but are defective in its export. A variety of secondary ‘rescue’ mutations within cap can occur to reduce polysaccharide synthesis and restore normal organism appearance and colony morphology.
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Molecular characterization of a cluster of at least two glucosyltransferase genes in Streptococcus salivarius ATCC 25975
More LessSummary: The oral micro-organism Streptococcus salivarius ATCC 25975 synthesizes extracellular glucosyltransferases (GTFs) which polymerize the glucose moiety of sucrose into glucan polymers. Two separate genes encoding the activities of a GTF-I (a GTF that synthesizes an insoluble product) and a GTF-S (a GTF that synthesizes soluble product) were cloned into bacteriophage λL47.1. The inserts in the λ-clones were characterized by restriction mapping and Southern hybridization and were found to overlap, implying that the two genes lay very close to one another on the S. salivarius chromosome. Both genes were subcloned into phagemid vector pIBI30 where they were expressed at a high level. The GTF-I-encoding gene was named gtfJ and the GTF-S-encoding gene, gtfK. Nucleotide sequencing showed that gtfJ and most probably gtfK were closely related to the gtf genes of the mutans streptococci. Sequence alignment also indicated that gtfK lay very close to and downstream from gtfJ, and that both were transcribed in the same direction.
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Effects of antibiotics on the growth and morphology of Pasteurella multocida
More LessSummary: The effects of subminimal inhibitory concentrations (subMICs) of certain antibiotics, namely penicillin G, tetracycline and trimethoprim/sulphamethoxazole, on the growth and morphology of Pasteurella multocida were evaluated. SubMICs of penicillin markedly reduced the growth of P. multocida. Tetracycline and trimethoprim/ sulphamethoxazole had no effect on its growth. SubMICs of penicillin greatly affected the morphology of P. multocida. At the highest concentrations tested (1/2 and 1/4 MIC) cells were acapsulate, and long filamentous cells (4–6 μm) were observed with some isolates. There was no correlation between the observed differences in the penicillin-binding proteins of the P. multocida isolates, and the extent of cell filamentation induced by penicillin G. SubMICs of tetracycline and trimethoprim/sulphamethoxazole did not seem to affect capsule production although filamentation was observed. Our results indicate that subMICs of penicillin can reduce growth of P. multocida. Furthermore, results also indicate that subMICs of antibiotics can affect the production of capsular material and the morphology of P. multocida.
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- Physiology And Growth
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Relationship between threonine dehydratase and biosynthesis of tylosin in Streptomyces fradiae
More LessTo elucidate the repression mechanism of ammonium ions on the biosynthesis of tylosin in Streptomyces fradiae NRRL 2702, enzyme activities involved in the metabolism of the aspartate family of amino acids were evaluated in relation to the ammonium ion concentration and tylosin production. It was found that aspartate aminotransferase was essential for both cell growth and tylosin production. However, both threonine dehydratase and valine dehydrogenase were repressed by supplemented ammonium ions at concentrations higher than 50 mm. Threonine dehydratase was purified from cell-free extracts by acetone precipitation, ion-exchange chromatography and gel filtration, and its molecular mass was estimated to be 67200 Da. The optimum pH and temperature for threonine dehydratase activity were 7·5 and 25 °C, respectively, and the K m value for threonine under these optimum conditions was 21 mm. The inhibition pattern of ammonium ions on the activity of threonine dehydratase appeared to be a mixed type.
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Hyperpolarization and intracellular acidification in Trichoderma viride as a response to illumination
More LessUsing indirect methods based on uptake of [3H]tetraphenylphosphonium cation and [14C]benzoic acid by cells of the fungus Trichoderma viride we found that the illumination-induced transient hyperpolarization of the plasma membrane is followed immediately by a rapid temporary decrease in intracellular pH. Hyperpolarization and intracellular acidification were completely suppressed by 150 mm-KCI and by the K+-ionophore valinomycin. The light-induced acidification of the cytoplasm was not observed in the presence of the cytochrome respiratory chain inhibitors antimycin A and mucidin. Based on these results, we hypothesize that the hyperpolarization of the cells is the consequence of an efflux of K+ through a light-activated K+-channel in the plasma membrane. The loss of positive charge in the cytoplasm caused by this efflux of cations is counterbalanced by H+ originating from the light-activated mitochondrial respiratory chain.
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Regulation of compatible solute accumulation in Salmonella typhimurium: evidence for a glycine betaine efflux system
More LessThe regulation of glycine betaine accumulation has been investigated in Salmonella typhimurium. The size of the glycine betaine pool in the cells is determined by the external osmotic pressure and is largely independent of the external glycine betaine concentration. Analysis of the activity of the ProP and ProU transport systems suggests that other systems must be active in the regulation of the glycine betaine pool. Addition of p-chloromercuribenzoate (PCMB) or p-chloromercuribenzene sulphonate (PCMBS) to cells that have accumulated glycine betaine provokes rapid loss of glycine betaine. The route of glycine betaine efflux under the influence of PCMB is independent of either the ProP or ProU transport systems. Rapid loss of the accumulated pool of glycine betaine in the presence of PCMB is specific to glycine betaine and proline; accumulated pools of serine and lysine are not significantly affected by the –SH reagent. A specific glycine betaine/proline efflux system is postulated on the basis of these data and its role in the regulation of glycine betaine and proline accumulation is discussed.
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