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枯草芽孢杆菌的CsrA通过阻断核糖体结合来调节鞭毛蛋白基因(hag)编码的翻译起始。

CsrA of Bacillus subtilis regulates translation initiation of the gene encoding the flagellin protein (hag) by blocking ribosome binding.

作者信息

Yakhnin Helen, Pandit Pallavi, Petty Tom J, Baker Carol S, Romeo Tony, Babitzke Paul

机构信息

Department of Biochemistry and Molecular Biology, The Pennsylvania State University, University Park, PA 16802, USA.

出版信息

Mol Microbiol. 2007 Jun;64(6):1605-20. doi: 10.1111/j.1365-2958.2007.05765.x.

DOI:10.1111/j.1365-2958.2007.05765.x
PMID:17555441
Abstract

The global regulatory Csr (carbon storage regulator) and the homologous Rsm (repressor of secondary metabolites) systems of Gram-negative bacteria typically consist of an RNA-binding protein (CsrA/RsmA) and at least one sRNA that functions as a CsrA antagonist. CsrA modulates gene expression post-transcriptionally by regulating translation initiation and/or mRNA stability of target transcripts. While Csr has been extensively studied in Gram-negative bacteria, until now Csr has not been characterized in any Gram-positive organism. csrA of Bacillus subtilis is the last gene of a flagellum biosynthetic operon. In addition to the previously identified sigma(D)-dependent promoter that controls expression of the entire operon, a sigma(A)-dependent promoter was identified that temporally controls expression of the last two genes of the operon (fliW-csrA); expression peaks 1 h after cell growth deviates from exponential phase. hag, the gene encoding flagellin, was identified as a CsrA-regulated gene. CsrA was found to repress hag'-'lacZ expression, while overexpression of csrA reduces cell motility. In vitro binding studies identified two CsrA binding sites in the hag leader transcript, one of which overlaps the hag Shine-Dalgarno sequence. Toeprint and cell-free translation studies demonstrate that bound CsrA prevents ribosome binding to the hag transcript, thereby inhibiting translation initiation and Hag synthesis.

摘要

革兰氏阴性菌的全局调控Csr(碳储存调控因子)和同源Rsm(次生代谢产物阻遏物)系统通常由一种RNA结合蛋白(CsrA/RsmA)和至少一种作为CsrA拮抗剂发挥作用的小RNA组成。CsrA通过调节靶转录本的翻译起始和/或mRNA稳定性在转录后调节基因表达。虽然Csr在革兰氏阴性菌中已得到广泛研究,但迄今为止在任何革兰氏阳性生物中尚未对Csr进行表征。枯草芽孢杆菌的csrA是鞭毛生物合成操纵子的最后一个基因。除了先前鉴定的控制整个操纵子表达的依赖于sigma(D)的启动子外,还鉴定了一个依赖于sigma(A)的启动子,该启动子在时间上控制操纵子最后两个基因(fliW-csrA)的表达;在细胞生长偏离指数期1小时后表达达到峰值。编码鞭毛蛋白的hag基因被鉴定为受CsrA调控的基因。发现CsrA抑制hag'-'lacZ表达,而csrA的过表达会降低细胞运动性。体外结合研究在hag前导转录本中鉴定出两个CsrA结合位点,其中一个与hag的Shine-Dalgarno序列重叠。足迹法和无细胞翻译研究表明,结合的CsrA可阻止核糖体与hag转录本结合,从而抑制翻译起始和Hag合成。

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