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全局调控因子σS和Lrp、特异性抑制剂CbpM以及CbpM的蛋白水解降解对DnaJ同源物CbpA的复杂调控。

Complex regulation of the DnaJ homolog CbpA by the global regulators sigmaS and Lrp, by the specific inhibitor CbpM, and by the proteolytic degradation of CbpM.

作者信息

Chenoweth Matthew R, Wickner Sue

机构信息

Laboratory of Molecular Biology, National Cancer Institute, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

J Bacteriol. 2008 Aug;190(15):5153-61. doi: 10.1128/JB.00437-08. Epub 2008 May 23.

Abstract

CbpA is a DnaJ homolog that functions as a DnaK cochaperone. Several cellular processes, including growth at low and high temperatures and septum formation during cell division, require either CbpA or DnaJ. CbpA is encoded in an operon with the gene for CbpM, which is a specific in vivo and in vitro inhibitor of CbpA. Here, we have cooverexpressed CbpA with CbpM in a DeltacbpAM DeltadnaJ strain and examined the resulting phenotypes. Under these conditions, sufficient free CbpA activity was present to support growth at low temperatures, but not at high temperatures. Defects in cell division and in lambda replication were also partially complemented by CbpA when cooverexpressed with CbpM. Utilizing reporter fusions, we demonstrated that the cbpAM operon was maximally transcribed at the transition from exponential growth to stationary phase. Transcription was controlled by the sigma(S) and Lrp global regulators, and both leucine availability and growth temperature influenced transcription. CbpA and CbpM accumulated to similar levels in stationary phase, approximately 2,300 monomers per cell. When not bound to CbpA, CbpM was unstable and was degraded by the Lon and ClpAP proteases. These data demonstrate that CbpA activity is controlled at multiple levels.

摘要

CbpA是一种DnaJ同源物,作为DnaK的共伴侣发挥作用。包括在低温和高温下生长以及细胞分裂过程中的隔膜形成在内的几个细胞过程,都需要CbpA或DnaJ。CbpA与CbpM基因一起编码在一个操纵子中,CbpM是CbpA在体内和体外的特异性抑制剂。在这里,我们在缺失CbpAM和缺失DnaJ的菌株中共同过量表达CbpA和CbpM,并检查了产生的表型。在这些条件下,存在足够的游离CbpA活性来支持低温下的生长,但不能支持高温下的生长。当与CbpM共同过量表达时,CbpA也部分弥补了细胞分裂和λ复制中的缺陷。利用报告基因融合,我们证明了cbpAM操纵子在从指数生长到稳定期的转变过程中转录达到最大值。转录受全局调节因子sigma(S)和Lrp控制,亮氨酸可用性和生长温度都影响转录。CbpA和CbpM在稳定期积累到相似水平,每个细胞约2300个单体。当不与CbpA结合时,CbpM不稳定,会被Lon和ClpAP蛋白酶降解。这些数据表明CbpA的活性在多个水平上受到控制。

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