Involvement of Clp protease activity in modulating the Bacillus subtilis σW stress response

被引:52
|
作者
Zellmeier, Stephan [1 ]
Schumann, Wolfgang [1 ]
Wiegert, Thomas [1 ]
机构
[1] Univ Bayreuth, Inst Genet, D-95440 Bayreuth, Germany
关键词
GENE-EXPRESSION; PROTEOLYSIS; SIGNAL; BIOSYNTHESIS; RESTRICTION; DEGRADATION; COMPETENCE; PROMOTERS; REGULATOR; PEPTIDASE;
D O I
10.1111/j.1365-2958.2006.05323.x
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The induction of Bacillus subtilis genes controlled by the extracytoplasmic function alternative sigma factor sigma(W) is strongly impaired in a strain deleted for the ClpP peptidase gene and in a double knockout of the ClpX and ClpE ATPase genes. Truncated soluble forms of the sigma(W) anti-sigma factor RsiW are stabilized in a clpP minus strain as revealed by the green fluorescent reporter protein fused to the N-terminus of RsiW and by pulse-chase experiments. Conserved alanine residues are present in the transmembrane region of RsiW, and mutations in these positions abolish induction of sigma(W)-controlled genes. Following alkaline shock, a truncated cytoplasmic form of RsiW is detectable in a strain expressing a triple alanine mutant allele of rsiW. These data point to a mechanism where the trans-membrane segment of RsiW contains a cryptic proteolytic tag that is uncovered as a result of intramembrane proteolysis of RsiW by RasP (YluC). After RasP-clipped RsiW is detached from the membrane, this proteolytic tag becomes crucial for the complete degradation of RsiW by cytoplasmic proteases and the release of sigma(W). ClpXP plays a major role in this third proteolytic step of stress-induced degradation of RsiW. Overexpression of SsrA-tagged green fluorescent protein as a ClpXP substrate protein reduces alkali induction of a sigma(W)-controlled gene by a factor of about three, indicating that a titration mechanism is able to tune the sigma(W)-mediated stress response to the cellular state.
引用
收藏
页码:1569 / 1582
页数:14
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