CcpA通过一个新的转录起始位点P(A6)导致phoPR启动子的抑制。
CcpA causes repression of the phoPR promoter through a novel transcription start site, P(A6).
作者信息
Puri-Taneja Ankita, Paul Salbi, Chen Yinghua, Hulett F Marion
机构信息
Laboratory for Molecular Biology, Department of Biological Sciences, University of Illinois at Chicago, 900 S. Ashland Ave. (M/C 567), Chicago, Illinois 60607, USA.
出版信息
J Bacteriol. 2006 Feb;188(4):1266-78. doi: 10.1128/JB.188.4.1266-1278.2006.
The Bacillus subtilis PhoPR two-component system is directly responsible for activation or repression of Pho regulon genes in response to phosphate deprivation. The response regulator, PhoP, and the histidine kinase, PhoR, are encoded in a single operon with a complex promoter region that contains five known transcription start sites, which respond to at least two regulatory proteins. We report here the identification of another direct regulator of phoPR transcription, carbon catabolite protein A, CcpA. This regulator functions in the presence of glucose or other readily metabolized carbon sources. The maximum derepression of phoPR expression in a ccpA mutant compared to a wild-type stain was observed under excess phosphate conditions with glucose either throughout growth in a high-phosphate defined medium or in a low-phosphate defined medium during exponential growth, a growth condition when phoPR transcription is low in a wild-type strain due to the absence of autoinduction. Either HPr or Crh were sufficient to cause CcpA dependent repression of the phoPR promoter in vivo. A ptsH1 (Hpr) crh double mutant completely relieves phoPR repression during phosphate starvation but not during phosphate replete growth. In vivo and in vitro studies showed that CcpA repressed phoPR transcription by binding directly to the cre consensus sequence present in the promoter. Primer extension and in vitro transcription studies revealed that the CcpA regulation of phoPR transcription was due to repression of P(A6), a previously unidentified promoter positioned immediately upstream of the cre box. Esigma(A) was sufficient for transcription of P(A6), which was repressed by CcpA in vitro. These studies showed direct repression by CcpA of a newly discovered Esigma(A)-responsive phoPR promoter that required either Hpr or Crh in vivo for direct binding to the putative consensus cre sequence located between P(A6) and the five downstream promoters characterized previously.
枯草芽孢杆菌的PhoPR双组分系统直接负责响应磷酸盐剥夺激活或抑制Pho调控子基因。响应调节因子PhoP和组氨酸激酶PhoR编码在一个具有复杂启动子区域的单一操纵子中,该启动子区域包含五个已知的转录起始位点,这些位点对至少两种调节蛋白有反应。我们在此报告了另一种phoPR转录的直接调节因子,即碳分解代谢物蛋白A(CcpA)的鉴定。该调节因子在葡萄糖或其他易于代谢的碳源存在时发挥作用。与野生型菌株相比,在ccpA突变体中,phoPR表达的最大去抑制作用在过量磷酸盐条件下观察到,即在高磷酸盐限定培养基中整个生长过程中或在指数生长期间的低磷酸盐限定培养基中添加葡萄糖时,在野生型菌株中,由于缺乏自诱导,phoPR转录在这种生长条件下较低。HPr或Crh足以在体内引起CcpA依赖的phoPR启动子抑制。ptsH1(Hpr)crh双突变体在磷酸盐饥饿期间完全解除phoPR抑制,但在磷酸盐充足生长期间则不然。体内和体外研究表明,CcpA通过直接结合启动子中存在的cre共有序列来抑制phoPR转录。引物延伸和体外转录研究表明,CcpA对phoPR转录的调节是由于对P(A6)的抑制,P(A6)是位于cre框上游紧邻的一个先前未鉴定的启动子。Eσ(A)足以用于P(A6)的转录,P(A6)在体外被CcpA抑制。这些研究表明,CcpA直接抑制新发现的Eσ(A)响应性phoPR启动子,该启动子在体内需要Hpr或Crh直接结合到位于P(A6)和先前表征的五个下游启动子之间的假定共有cre序列。
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