- Volume 31, Issue 2, 1990
Volume 31, Issue 2, 1990
- Review Article
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A comparison of specificity and biological activity of polyclonal and monoclonal antibodies raised against Salmonella minnesota R595 lipopolysaccharide
More LessSummaryMurine monoclonal antibodies (MAbs) and immune rabbit serum were raised against the rough mutant of Salmonella minnesota strain R595. These antibodies were tested for their ability to inhibit LPS-induced B-cell mitogenicity and neutralise LPS toxicity in chick embryos. Immune rabbit serum inhibited both mitogenicity and LPS lethality. None of the MAbs or a cocktail of antibodies were able to neutralise LPS lethality in chick embryos. However, they were able to inhibit mitogenicity by varying degrees.
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Protective immunity induced in mice by detoxified salmonella lipopolysaccharide
More LessSummaryC3H/HeNMTV mice were immunised intraperitoneally (i.p.) with lipopolysaccharide (LPS) or detoxified LPS (D-LPS) derived from Salmonella typhimurium strain SR-11. In both cases, effective protection was achieved against a challenge dose of greater than 2x102 LD50 of the same organism given by i.p. injection. However, by comparison with LPS, approximately 6- to 10-fold more of D-LPS by weight was needed to protect mice to an equivalent degree. Histopathological studies showed that the initial lesions in infected mice protected with either LPS or D-LPS were composed of self-limiting abscesses which transformed into granulomas as the animals recovered. It is suggested that D-LPS may be modified to become a highly effective, non-toxic salmonella vaccine.
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Pathogenic potential of Eubacterium yurii subspecies
More LessSummarySeveral mechanisms that could contribute to the periodontopathogenic potential of Eubacterium yurii were investigated. All 18 strains examined produced RNAase and the metabolites H2S, indole and butyrate. Some strains produced phosphatase and DNAase. Methanol extracts of whole cells of E. yurii subspp. yurii and margaretiae stimulated bone resorption in vitro comparable to that produced by recognised periodontal pathogens. These results suggest that further studies should be performed to elucidate the role of E. yurii in periodontal disease.
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Survival of Pseudomonas pseudomallei in human phagocytes
More LessSummaryPseudomonas pseudomallei causes the disease melioidosis, with protean manifestations, protracted clinical course and unpredictable response to antimicrobial treatment. Intracellular location of the organism is suspected to be the cause of these properties. This study was undertaken to examine the intracellular growth of this bacterium. Intracellular growth and survival was assessed at different time intervals, by Gram´s stain and electronmicroscopic examination. During the first 5 h, the numbers of P. pseudomallei within phagocytes did not change significantly. By 18-21 h, gram-stained preparations revealed that P. pseudomallei cells completely filled the phagocytes and electronmicroscopy showed evidence of binary fission. During that time the number of cfu of P. pseudomallei growing simultaneously in vitro increased by log10 2-3. The phagocytes remained viable throughout the observation period and retained their capacity to produce an oxidative burst for the first hour of incubation. The ability of P. pseudomallei to survive and multiply in phagocytes shows that it is a facultative intracellular bacterium. This finding is relevant to the selection of antimicrobial regimens, and the management of the disease.
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Chromosomal aberrations in germ cells of male mice immunised with attenuated viral vaccines (human)
More LessSummaryThe cytogenetic effects of two attenuated viral vaccines (yellow fever vaccine and oral poliomyelitis vaccine) were assessed by means of the analysis of meiotic spermatocyte chromosomes in mice. In a dose of 0.5 ml, but not 0.1 ml, both vaccines induced a significant percentage of chromosomal aberrations after 7, 14 and 30 days. Euploidy was the major abnormality produced by yellow fever vaccine. The various abnormalities produced by oral polio vaccine were significant when pooled, but not when analysed individually. More abnormalities were produced by yellow fever vaccine than by oral polio vaccine.
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Ecology of Pseudomonas aeruginosa in patients with cystic fibrosis
SummaryThe occurrence of various Pseudomonas aeruginosa strains in the sputum of 15 patients with cystic fibrosis (CF) was monitored over periods ranging from 2 to 60 months. Isolates of P. aeruginosa were typed by four different techniques, namely serotyping, active and passive pyocin typing, and phage typing. The maximum number of different serotypes found in the patients was three (one serotype in nine patients; two serotypes in five patients; three serotypes in one patient). Pyocin and phage typing showed no marked differences between strains of the same serotype in individual patients. Exacerbations of chronic respiratory infection were not associated with changes in the sputum flora, the composition of P. aeruginosa strains in which remains constant over long periods in patients with CF.
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- Articles
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Long-term viability of stored mycoplasmas and ureaplasmas
More LessSummaryAll of five lyophilised cultures of Mycoplasma orale kept for 23 years at room temperature were still viable, as were all but one of 12 lyophilised cultures of six Mycoplasma spp. that had been stored for 18–22 years at 4°C. Similarly, 11 of 13 lyophilised ureaplasma cultures were viable after 8–22 years at 4°C; the titre of organisms in the viable cultures had diminished no more than 100-fold, Seven broth cultures of five different Mycoplasma spp. all proved viable 5-13 years after being frozen and stored at — 70°C, although there was up to 104-fold reduction in the titre of organisms in some cultures. Furthermore, 18 (82%) of 22 different Mycoplasmaspp., originally lyophilised and then reconstituted and stored at — 70°C, were viable after 16 years. Viable organisms were found, with little or no reduction in titre, in all of seven broth cultures of Ureaplasma urealyticum, comprising six serotypes, after storage for 6-10 years at — 70°C, but five of 18 broth cultures of other human and animal ureaplasmas stored likewise were not viable after 13-14 years and in a further seven of them the titre of viable organisms had diminished ≥ 104-fold.
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- Review Article
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Characterisation of methicillin-resistant Staphylococcus aureus by biotyping, immunoblotting and restriction enzyme fragmentation patterns
More LessSummaryWe have characterised 45 isolates of methicillin-resistant Staphylococcus aureus (MRSA) from Glasgow Royal Infirmary by means of simple biotyping, immunoblotting of exported proteins and restriction enzyme fragmentation patterns (REFP) of plasmid DNA. The strains were subdivided into four groups (A-D) on the basis of biotype. Immunoblotting and restriction enzyme fragmentation generated a number of unique patterns. Analysis of these patterns by means of Dice coefficients of similarity separated them into two major immunoblot groups (Blot1 and Blot2) and two major REFP groups (FP1 and FP2). There was strong positive correlation between Blot1 and FP1 groups and between Blot2 and FP2 groups. In addition, Blot1-FP1 isolates were almost exclusively of biotypes A or C, whereas Blot2-FP2 isolates were of biotypes B or D. The methods described here have provided comprehensive epidemiological information which has been valuable in studying the origin and spread of MRSA.
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- Articles
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A new class of conjugative plasmid in Staphylococcus aureus
E. E. Udo and W. B. GrubbSummaryPlasmid pWBG637, a Staphylococcus aureus conjugative plasmid having no known resistance phenotype, was compared with other conjugative plasmids in S. aureus by restriction endonuclease analysis, incompatibility testing and DNA-DNA hybridisation. It differed from the other conjugative plasmids on all three criteria and thus belongs to a new class of conjugative plasmids.
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- Review Article
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A rapid technique for detection of resistance to chloramphenicol in Streptococcus pneumoniae and comparison with minimum inhibitory concentration and disk-diffusion methods
More LessSummaryFifty-two strains of Streptococcus pneumoniae were examined for production of chloramphenicol acetyltransferase (CAT) by a rapid technique based upon induction of enzyme activity and chemical assay. This method was compared with one measuring the minimum inhibitory concentration (MIC) by agar dilution and a diffusion test with disks containing 10 μg, 30 μg and 50 μg of chloramphenicol. The MIC for 13 chloramphenicol-resistant strains was 16 mg/L and for 39 sensitive strains ≤4 mg/L. The chemical assay clearly distinguished resistant from sensitive strains; it was technically simple and provided results within 90 min. The distinction between sensitive and resistant bacteria in the disk diffusion assay was clearer with 10-μg than with 30-μg and 50-μg disks. However, the chemical CAT assay, with enzyme induction, is recommended when a rapid result is required.
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A pyrolysis-mass spectrometry study of Corynebacterium spp.
More LessSummaryClinical (66) and collection (38) strains of Corynebacterium spp., including C. jeikeium and CDC group D2, and of Listeria monocytogenes were examined. Conventional characters used in species identification were assessed by a micro-biochemical method, and pyrolysis-mass spectrometry (Py-MS) was performed with a Horizon Instruments PYMS 200X. Classification based on Py-MS data yielded clusters that corresponded with species identification and classification groups from conventional data. One small group of clinical strains, homogeneous in conventional tests and Py-MS, comprised isolates from sputum samples from patients undergoing ventilation; they were similar to collection strains of C. renale and C. striatum; the latter species has been implicated in chest infection. Another group, similar to C. minutissimum in both systems, comprised clinical strains isolated from urogenital specimens. L. monocytogenes strains were clearly distinct from Corynebacterium spp. Groups comprising CDC D2 strains and C. jeikeium were resolved, and were similar to other Corynebacterium spp. Two collection strains of C. xerosis were distinct in conventional tests and Py-MS.
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