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SecB表达的分解代谢阻遏在转录水平上由环腺苷酸(cAMP)受体蛋白 - cAMP复合物正向调控。

Catabolic repression of secB expression is positively controlled by cyclic AMP (cAMP) receptor protein-cAMP complexes at the transcriptional level.

作者信息

Seoh H K, Tai P C

机构信息

Department of Biology, Georgia State University, Atlanta, Georgia 30303, USA.

出版信息

J Bacteriol. 1999 Mar;181(6):1892-9. doi: 10.1128/JB.181.6.1892-1899.1999.

Abstract

SecB, a protein export-specific chaperone, enhances the export of a subset of proteins across cytoplasmic membranes of Escherichia coli. Previous studies showed that the synthesis of SecB is repressed by the presence of glucose in the medium. The derepression of SecB requires the products of both the cya and crp genes, indicating that secB expression is under the control of catabolic repression. In this study, two secB-specific promoters were identified. In addition, 5' transcription initiation sites from these two promoters were determined by means of secB-lacZ fusions and primer extension. The distal P1 promoter appeared to be independent of carbon sources, whereas the proximal P2 promoter was shown to be subject to control by the cyclic AMP (cAMP) receptor protein (CRP)-cAMP complexes. Gel-mobility shift studies showed that this regulation results from direct interaction between the secB P2 promoter region and the CRP-cAMP complex. Moreover, the CRP binding site on the secB gene was determined by DNase I footprinting and further substantiated by mutational analysis. The identified secB CRP binding region is centered at the -61.5 region of the secB gene and differed from the putative binding sites predicted by computer analysis.

摘要

SecB是一种蛋白质输出特异性伴侣蛋白,可促进大肠杆菌细胞质膜上一部分蛋白质的输出。先前的研究表明,培养基中葡萄糖的存在会抑制SecB的合成。SecB的去阻遏需要cya和crp基因的产物,这表明secB的表达受分解代谢阻遏的控制。在本研究中,鉴定出了两个secB特异性启动子。此外,通过secB - lacZ融合和引物延伸确定了这两个启动子的5'转录起始位点。远端的P1启动子似乎与碳源无关,而近端的P2启动子则受环腺苷酸(cAMP)受体蛋白(CRP)- cAMP复合物的控制。凝胶迁移率变动研究表明,这种调控是由secB P2启动子区域与CRP - cAMP复合物之间的直接相互作用引起的。此外,通过DNase I足迹法确定了secB基因上的CRP结合位点,并通过突变分析进一步证实。鉴定出的secB CRP结合区域位于secB基因的 - 61.5区域,与计算机分析预测的假定结合位点不同。

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