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来自肠致病性大肠杆菌的一种AraC样蛋白PerA对毒力基因的直接和间接转录激活作用。

Direct and indirect transcriptional activation of virulence genes by an AraC-like protein, PerA from enteropathogenic Escherichia coli.

作者信息

Porter Megan E, Mitchell Paul, Roe Andrew J, Free Andrew, Smith David G E, Gally David L

机构信息

Zoonotic and Animal Pathogens Research Laboratory, Medical Microbiology, University of Edinburgh, Teviot Place, Edinburgh, EH8 9AG, UK.

出版信息

Mol Microbiol. 2004 Nov;54(4):1117-33. doi: 10.1111/j.1365-2958.2004.04333.x.

DOI:10.1111/j.1365-2958.2004.04333.x
PMID:15522091
Abstract

The plasmid-encoded Per regulatory locus of enteropathogenic Escherichia coli (EPEC) is generally considered to consist of three genes, perA, perB and perC. PerA, a member of the AraC-like family of transcriptional regulators, is known to be an activator of its own promoter (autoactivation) as well as of the plasmid-located bfp operon encoding bundle-forming pili, but its role in activation of the chromosomal locus of enterocyte effacement (LEE) pathogenicity island, which confers the property of intimate adherence on EPEC, requires clarification. Here, we show that PerA is also required for activation of the master regulatory LEE operon, LEE1, but that this activation is indirect, being achieved via autoactivation of the per promoter which ensures sufficient production of the PerC protein to activate LEE1. In contrast, PerA-dependent activation of the per and bfp promoters is direct and does not require the other Per proteins, but is modulated by the nucleoid-associated protein H-NS. The closely related VirF regulator from Shigella flexneri cannot substitute for PerA to activate these promoters, despite being able to bind their upstream regions in vitro. PerA can bind the per and bfp promoter fragments to form multiple complexes, while VirF forms only a single complex. Site-directed mutagenesis of the PerA protein suggests that, like VirF, it may use both of its carboxy-terminal helix-turn-helix motifs for DNA interaction, and may also make direct contacts with RNA polymerase. In addition, we have isolated mutations in the poorly characterized amino-terminal domain of PerA which affect its ability to activate gene expression.

摘要

肠致病性大肠杆菌(EPEC)的质粒编码Per调控位点通常被认为由三个基因组成,即perA、perB和perC。PerA是AraC样转录调节因子家族的成员,已知它是其自身启动子(自激活)以及编码束状菌毛的质粒定位bfp操纵子的激活因子,但其在激活赋予EPEC紧密黏附特性的肠细胞脱落(LEE)致病岛染色体位点中的作用尚需阐明。在此,我们表明PerA也是主调控LEE操纵子LEE1激活所必需的,但这种激活是间接的,是通过per启动子的自激活实现的,该自激活确保足够量的PerC蛋白产生以激活LEE1。相比之下,PerA对per和bfp启动子的依赖性激活是直接的,不需要其他Per蛋白,但受到类核相关蛋白H-NS的调节。尽管弗氏志贺菌密切相关的VirF调节因子在体外能够结合这些启动子的上游区域,但它不能替代PerA来激活这些启动子。PerA可以结合per和bfp启动子片段形成多个复合物,而VirF仅形成单个复合物。PerA蛋白的定点诱变表明,与VirF一样,它可能利用其两个羧基末端的螺旋-转角-螺旋基序进行DNA相互作用,并且也可能与RNA聚合酶直接接触。此外,我们在PerA特征不明确的氨基末端结构域中分离出了影响其激活基因表达能力的突变。

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