σ B Modulates Virulence Determinant Expression and Stress Resistance: Characterization of a Functional rsbU Strain Derived from Staphylococcus aureus 8325-4

Author:

Horsburgh Malcolm J.1,Aish Joanne L.1,White Ian J.1,Shaw Les1,Lithgow James K.1,Foster Simon J.1

Affiliation:

1. Department of Molecular Biology and Biotechnology, University of Sheffield, Western Bank, Sheffield, England S10 2TN

Abstract

ABSTRACT The accessory sigma factor σ B controls a general stress response that is thought to be important for Staphylococcus aureus survival and may contribute to virulence. The strain of choice for genetic studies, 8325-4, carries a small deletion in rsbU , which encodes a positive regulator of σ B activity. Consequently, to enable the role of σ B in virulence to be addressed, we constructed an rsbU + derivative, SH1000, using a method that does not leave behind an antibiotic resistance marker. The phenotypic properties of SH1000 (8325-4 rsbU + ) were characterized and compared to those of 8325-4, the rsbU mutant, parent strain. A recognition site for σ B was located in the promoter region of katA , the gene encoding the sole catalase of S. aureus , by primer extension analysis. However, catalase expression and activity were similar in SH1000 (8325-4 rsbU + ), suggesting that this promoter may have a minor role in catalase expression under normal conditions. Restoration of σ B activity in SH1000 (8325-4 rsbU + ) resulted in a marked decrease in the levels of the exoproteins SspA and Hla, and this is likely to be mediated by reduced expression of agr in this strain. By using Western blotting and a sarA-lacZ reporter assay, the levels of SarA were found to be similar in strains 8325-4 and SH1000 (8325-4 rsbU + ) and sigB mutant derivatives of these strains. This finding contrasts with previous reports that suggested that SarA expression levels are altered when they are measured transcriptionally. Inactivation of sarA in each of these strains resulted in an expected decrease in agr expression; however, the relative level of agr in SH1000 (8325-4 rsbU + ) remained less than the relative levels in 8325-4 and the sigB mutant derivatives. We suggest that SarA is not likely to be the effector in the overall σ B -mediated effect on agr expression.

Publisher

American Society for Microbiology

Subject

Molecular Biology,Microbiology

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