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肠致病性大肠杆菌(EPEC)LEE1 P1 启动子的一个不寻常特征。

An unusual feature associated with LEE1 P1 promoters in enteropathogenic Escherichia coli (EPEC).

机构信息

Center for Host Defense against Enteropathogenic Bacteria Infection, Department of Microbiology, Chonnam National University Medical School, Kwangju, South Korea.

出版信息

Mol Microbiol. 2012 Feb;83(3):612-22. doi: 10.1111/j.1365-2958.2011.07956.x. Epub 2012 Jan 9.

Abstract

Transcription start points in bacteria are influenced by the nature of the RNA polymerase·promoter interaction. For Escherichia coli RNA polymerase holoenzyme containing σ70, it is presumed that specific sequence in one or more of the -10, extended -10 and -35 elements of the promoter guides the RNAP to select the cognate start point. Here, we investigated the promoter driving expression of the LEE1 operon in enteropathogenic E. coli and found two promoters separated by 10 bp, LEE1 P1A (+1) and LEE1 P1B (+10) using various in vitro biochemical tools. A unique feature of P1B was the presence of multiple transcription starts from five neighbouring As at the initial transcribed region. The multiple products did not arise from stuttering synthesis. Analytical software based on information theory was employed to determine promoter elements. The concentration of the NTP pool altered the preferred transcription start points, albeit the underlying mechanism is elusive. Under in vivo conditions, dominant P1B, but not P1A, was subject to regulation by IHF.

摘要

细菌中转录起始点受 RNA 聚合酶·启动子相互作用的影响。对于含有 σ70 的大肠杆菌 RNA 聚合酶全酶,假定启动子的-10、延伸-10 和-35 元件中的一个或多个特定序列指导 RNAP 选择同源起始点。在这里,我们使用各种体外生化工具研究了肠致病性大肠杆菌中 LEE1 操纵子的启动子驱动表达,并发现了两个相隔 10bp 的启动子,LEE1 P1A(+1)和 LEE1 P1B(+10)。P1B 的一个独特特征是在初始转录区的五个相邻 As 处存在多个转录起始。这些多个产物不是由于停滞合成而产生的。基于信息理论的分析软件用于确定启动子元件。核苷酸池的浓度改变了首选的转录起始点,尽管其潜在机制尚不清楚。在体内条件下,主要的 P1B 而不是 P1A 受到 IHF 的调节。

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