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大肠杆菌中用于苯乙酸降解的双向paa分解代谢操纵子的转录调控。

Transcriptional regulation of the divergent paa catabolic operons for phenylacetic acid degradation in Escherichia coli.

作者信息

Ferrández A, García J L, Díaz E

机构信息

Department of Molecular Microbiology, Centro de Investigaciones Biológicas, Consejo Superior de Investigaciones Científicas, 28006 Madrid, Spain.

出版信息

J Biol Chem. 2000 Apr 21;275(16):12214-22. doi: 10.1074/jbc.275.16.12214.

DOI:10.1074/jbc.275.16.12214
PMID:10766858
Abstract

The expression of the divergently transcribed paaZ and paaABCDEFGHIJK catabolic operons, which are responsible for phenylacetic acid (PA) degradation in Escherichia coli, is driven by the Pz and Pa promoters, respectively. To study the transcriptional regulation of the inducible paa catabolic genes, genetic and biochemical approaches were used. Gel retardation assays showing that the PaaX regulator binds specifically to the Pa and Pz promoters were complemented with in vivo experiments that indicated a PaaX-mediated repression effect on the expression of Pa-lacZ and Pz-lacZ reporter fusions. The region within the Pa and Pz promoters that is protected by the PaaX repressor in DNase I footprinting assays contains a conserved 15-base pair imperfect palindromic sequence motif that was shown, through mutational analysis, to be indispensable for PaaX binding and repression. PA-coenzyme A (PA-CoA), but not PA, specifically inhibited binding of PaaX to the target sequences, thus confirming the first intermediate of the pathway as the true inducer and PaaX as the only bacterial regulatory protein described so far that responds to an aryl-CoA compound. Superimposed in the specific PaaX-mediated regulation is transcriptional activation by the cAMP receptor protein and the integration host factor protein. These global regulators may adjust the transcriptional output from Pa and Pz promoters to the overall growth status of the cell.

摘要

在大肠杆菌中负责苯乙酸(PA)降解的反向转录的paaZ和paaABCDEFGHIJK分解代谢操纵子的表达,分别由Pz和Pa启动子驱动。为了研究可诱导的paa分解代谢基因的转录调控,采用了遗传学和生物化学方法。凝胶阻滞试验表明PaaX调节因子与Pa和Pz启动子特异性结合,体内实验对其进行了补充,体内实验表明PaaX对Pa-lacZ和Pz-lacZ报告基因融合体的表达具有介导的抑制作用。在DNase I足迹试验中,PaaX阻遏物保护的Pa和Pz启动子区域包含一个保守的15个碱基对的不完全回文序列基序,通过突变分析表明,该基序对于PaaX结合和抑制是必不可少的。PA-辅酶A(PA-CoA)而非PA特异性抑制PaaX与靶序列的结合,从而证实该途径的第一个中间产物是真正的诱导物,PaaX是迄今为止描述的唯一对芳基-CoA化合物作出反应的细菌调节蛋白。在特定的PaaX介导的调控之上叠加的是由cAMP受体蛋白和整合宿主因子蛋白介导的转录激活。这些全局调节因子可能会根据细胞的整体生长状态调整Pa和Pz启动子的转录输出。

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