Affiliation:
1. Department of Microbiology, Molecular Biology and Biochemistry, University of Idaho, Moscow, Idaho 83844-3052
Abstract
ABSTRACT
Previous studies in our laboratory have shown that the
Staphylococcus aureus
LytSR two-component regulatory system affects murein hydrolase activity and autolysis. A LytSR-regulated dicistronic operon has also been identified and shown to encode two potential membrane-associated proteins, designated LrgA and LrgB, hypothesized to be involved in the control of murein hydrolase activity. In the present study, a
lrgAB
mutant strain was generated and analyzed to test this hypothesis. Zymographic and quantitative analysis of murein hydrolase activity revealed that the
lrgAB
mutant produced increased extracellular murein hydrolase activity compared to that of the wild-type strain. Complementation of the
lrgAB
defect by providing the
lrgAB
genes in
trans
restored the wild-type phenotype, indicating that these genes confer negative control on extracellular murein hydrolase activity. In addition to these effects, the influence of the
lrgAB
mutation on penicillin-induced lysis and killing was examined. These studies demonstrated that the
lrgAB
mutation enhanced penicillin-induced killing of cells approaching the stationary phase of growth, the time at which the
lrgAB
operon was shown to be maximally expressed. This effect of the
lrgAB
mutation on penicillin-induced killing was shown to be independent of cell lysis. In contrast, the
lrgAB
mutation did not affect penicillin-induced killing of cells growing in early-exponential phase, a time in which
lrgAB
expression was shown to be minimal. However, expression of the
lrgAB
operon in early-exponential-phase cells inhibited penicillin-induced killing, again independent of cell lysis. The data generated by this study suggest that penicillin-induced killing of
S. aureus
involves a novel regulator of murein hydrolase activity.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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