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Site-Specific Mutation of Staphylococcus aureus VraS Reveals a Crucial Role for the VraR-VraS Sensor in the Emergence of Glycopeptide Resistance
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ABSTRACT
An initial response of
Staphylococcus aureus
to encounter with cell wall-active antibiotics occurs by transmembrane signaling systems that orchestrate changes in gene expression to promote survival. Histidine kinase two-component sensor-response regulators such as VraRS contribute to this response. In this study, we examined VraS membrane sensor phosphotransfer signal transduction and explored the genetic consequences of disrupting signaling by engineering a site-specific
vraS
chromosomal mutation. We have used
in vitro
autophosphorylation assay with purified VraS[64-347] lacking its transmembrane anchor region and tested site-specific kinase domain histidine mutants. We identified VraS H156 as the probable site of autophosphorylation and show phosphotransfer
in vitro
using purified VraR. Genetic studies show that the
vraS
(
H156A
) mutation in three strain backgrounds (ISP794, Newman, and COL) fails to generate detectable first-step reduced susceptibility teicoplanin mutants and severely reduces first-step vancomycin mutants. The emergence of low-level glycopeptide resistance in strain ISP794, derived from strain 8325 (Δ
rsbU
), did not require a functional σ
B
, but
rsbU
restoration could enhance the emergence frequency supporting a role for this alternative sigma factor in promoting glycopeptide resistance. Transcriptional analysis of
vraS
(
H156A
) strains revealed a pronounced reduction but not complete abrogation of the
vraRS
operon after exposure to cell wall-active antibiotics, suggesting that additional factors independent of VraS-driven phosphotransfer, or σ
B
, exist for this promoter. Collectively, our results reveal important details of the VraRS signaling system and predict that pharmacologic blockade of the VraS sensor kinase will have profound effects on blocking emergence of cell wall-active antibiotic resistance in
S. aureus
.
American Society for Microbiology
Title: Site-Specific Mutation of
Staphylococcus aureus
VraS Reveals a Crucial Role for the VraR-VraS Sensor in the Emergence of Glycopeptide Resistance
Description:
ABSTRACT
An initial response of
Staphylococcus aureus
to encounter with cell wall-active antibiotics occurs by transmembrane signaling systems that orchestrate changes in gene expression to promote survival.
Histidine kinase two-component sensor-response regulators such as VraRS contribute to this response.
In this study, we examined VraS membrane sensor phosphotransfer signal transduction and explored the genetic consequences of disrupting signaling by engineering a site-specific
vraS
chromosomal mutation.
We have used
in vitro
autophosphorylation assay with purified VraS[64-347] lacking its transmembrane anchor region and tested site-specific kinase domain histidine mutants.
We identified VraS H156 as the probable site of autophosphorylation and show phosphotransfer
in vitro
using purified VraR.
Genetic studies show that the
vraS
(
H156A
) mutation in three strain backgrounds (ISP794, Newman, and COL) fails to generate detectable first-step reduced susceptibility teicoplanin mutants and severely reduces first-step vancomycin mutants.
The emergence of low-level glycopeptide resistance in strain ISP794, derived from strain 8325 (Δ
rsbU
), did not require a functional σ
B
, but
rsbU
restoration could enhance the emergence frequency supporting a role for this alternative sigma factor in promoting glycopeptide resistance.
Transcriptional analysis of
vraS
(
H156A
) strains revealed a pronounced reduction but not complete abrogation of the
vraRS
operon after exposure to cell wall-active antibiotics, suggesting that additional factors independent of VraS-driven phosphotransfer, or σ
B
, exist for this promoter.
Collectively, our results reveal important details of the VraRS signaling system and predict that pharmacologic blockade of the VraS sensor kinase will have profound effects on blocking emergence of cell wall-active antibiotic resistance in
S.
aureus
.
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