Affiliation:
1. Institut für Mikrobiologie, Ernst-Moritz-Arndt-Universität, 17487 Greifswald, Germany
2. Institute for Cell and Molecular Biosciences, Faculty of Medical Sciences, University of Newcastle, Newcastle upon Tyne NE2 4HH, United Kingdom
Abstract
ABSTRACT
SigB is an alternative sigma factor that controls a large regulon in
Staphylococcus aureus
. Activation of SigB requires RsbU, a protein phosphatase 2C (PP2C)-type phosphatase. In a closely related organism,
Bacillus subtilis
, RsbU activity is stimulated upon interaction with RsbT, a kinase, which following an activating stimulus switches from a 25S high-molecular-weight complex, the stressosome, to the N-terminal domain of RsbU. Active RsbU dephosporylates RsbV and thereby triggers the release of SigB from its inhibitory complex with RsbW. While RsbU, RsbV, RsbW, and SigB are conserved in
S. aureus
, proteins similar to RsbT and the components of the stressosome are not, raising the question of how RsbU activity and hence SigB activity are controlled in
S. aureus
. We found that in contrast to the case in
B. subtilis
, the induced expression of RsbU was sufficient to stimulate SigB-dependent transcription in
S. aureus
. However, activation of SigB-dependent transcription following alkaline stress did not lead to a clear accumulation of SigB and its regulators RsbV and RsbW or to a change in the RsbV/RsbV-P ratio in
S. aureus
. When expressed in
B. subtilis
, the
S. aureus
RsbU displayed a high activity even in the absence of an inducing stimulus. This high activity could be transferred to the PP2C domain of the
B. subtilis
RsbU protein by a fusion to the N-terminal domain of the
S. aureus
RsbU. Collectively, the data suggest that the activity of the
S. aureus
RsbU and hence SigB may be subjected to different regulation in comparison to that in
B. subtilis
.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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