M. A. Livesley scite author profile

A genomic DNA library of Staphylococcus epidermidis NCTC 11047 was constructed, using the Lambda Zap Express cloning vector, and screened with serum collected from a patient with S. epidermidis endocarditis. Sequence analysis of a 30 kDa cloned protein, termed staphylococcal secretory antigen, SsaA, identified a novel protein not previously reported in S. epidermidis. SsaA showed strong homology with two other staphylococcal proteins: SceB from Staphylococcus carnosus and a staphyloxanthin biosynthesis protein from Staphylococcus aureus. Further investigation revealed SsaA to be a highly antigenic protein that was expressed in vivo and could be recovered from whole cells and from the culture supernatant. A combination of Western blot analysis and PCR screening identified SsaA or a homologue in 103/103 staphylococcal strains. SsaA-like genes were not detected in other Gram-positive bacteria of medical importance or a number of Gram-negative organisms. Elevated anti-SsaA IgG antibody levels were detected in sera of five patients with S. epidermidis endocarditis but not in patients with other S. epidermidis infections, endocarditis of other aetiologies or patients with no evidence of infection. The expression of SsaA during episodes of S. epidermidis endocarditis suggests a virulence role specific to the pathogenesis of this infectious disease.

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Sub-specific differentiation of intestinal spirochaete isolates by macrorestriction fragment profiling

Rayment

Livesley

Barrett

1997

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Macrorestriction fragment profile analysis by PFGE was used to distinguish intestinal spirochaetes, some of which were isolated from cases of swine dysentery and intestinal spirochaetosis in humans, pigs, mice, chickens and dogs. Macrorestriction fragment profiles using SmaI and Sacll restriction enzymes were produced and used in statistical analysis. This permitted the division of the isolates into two major clusters. One cluster contained isolates which were identified as Sepulina pilosicoli and the second cluster contained isolates identified as Serpuline hyodysenteriae by immunoblotting with species-specific mAbs. Both species contained sub-specif ic groups, although these rarely correlated with the source of the isolates. We conclude that PFGE is capable of sub-specif ic differentiation of intestinal spirochaetes, but that the current species contain a large variety of genotypes among which crossspecies transmission may be feasible.

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The Effects of Ageing upon α-Amylase Production and Protein Synthesis by Wheat Aleurone Layers

Livesley

Bray

1991

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Use of pulsed field gel electrophoresis to determine the source of microbial contamination of central venous catheters

Livesley

Tebbs

Moss

et al. 1998

Eur. J. Clin. Microbiol. Infect. Dis.

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Microorganisms detected in situ on the distal tip of central venous catheters (CVC) within 90 min of insertion were investigated using pulsed-field gel electrophoresis to analyse genomic fragments obtained with the SmaI restriction enzyme. Thirty patients received a triple lumen CVC, which was inserted directly through the skin using the Seldinger technique. In a further 30 patients a triple lumen CVC was inserted through a Swan sheath, thereby avoiding direct contact of the CVC with the skin. Staphylococci were isolated from the distal tips of the catheters in 6 patients (5 who had the CVC inserted directly through the skin and 1 who had the CVC inserted via a Swan sheath.) Twenty-three staphylococcal isolates were also isolated from the insertion equipment and the skin swabs surrounding the insertion site of these six patients. All the isolates were genotyped. In one of the patients the organisms isolated from the skin were identical to those on the CVC tip. In two further patients similar organisms were isolated from the insertion equipment and the patients' skin. These results, in addition to the reduced colonisation rates observed when catheters were introduced through a Swan sheath, support the hypothesis that microorganisms from the skin are impacted onto the CVC tip and the CVC insertion equipment at catheter insertion.

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M. A. Livesley

The genomic diversity of coagulase- negative Staphylococci associated with nosocomial infections

Identification of a novel antigen fromStaphylococcus epidermidis

Sub-specific differentiation of intestinal spirochaete isolates by macrorestriction fragment profiling

The Effects of Ageing upon α-Amylase Production and Protein Synthesis by Wheat Aleurone Layers

Use of pulsed field gel electrophoresis to determine the source of microbial contamination of central venous catheters

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