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Fis对大肠杆菌拓扑异构酶I的差异调控

Differential regulation of Escherichia coli topoisomerase I by Fis.

作者信息

Weinstein-Fischer Dalit, Altuvia Shoshy

机构信息

Department of Molecular Genetics and Biotechnology, The Hebrew University-Hadassah Medical School, Jerusalem, Israel.

出版信息

Mol Microbiol. 2007 Feb;63(4):1131-44. doi: 10.1111/j.1365-2958.2006.05569.x.

Abstract

We previously reported that the P1 promoter of topA encoding topoisomerase I of Escherichia coli is activated in response to oxidative stress, in a Fis-dependent manner. Here we show that Fis regulation of topA varies with the intracellular concentrations of Fis. Thus, when Fis levels are low, hydrogen peroxide treatment results in topA activation, whereas at high Fis levels hydrogen peroxide treatment renders topA P1 inactive. In vivo DMS footprinting indicates that only at low Fis levels, when exposed to the stress, the region of the topA promoter changes and P1 becomes active. Potassium permanganate experiments indicate that low levels of Fis activate P1 transcription by facilitating the formation of open complexes, while high levels of this protein shut off the promoter. DNase I footprinting show that Fis binds the promoter region of topA at eight sites with different affinities. One low affinity site overlaps the -10, -35 hexamers of RNA polymerase. We propose that in response to oxidative stress, when present at low levels, Fis binds the promoter region of topA at its high affinity sites, thereby facilitating the recruitment of RNA polymerase to P1, while at high levels, Fis occupies the low affinity sites as well, and thus prevents the binding of RNA polymerase. Our results indicate that the oxidative stress response varies in response to changes in growth phase and nutritional environment.

摘要

我们先前报道过,编码大肠杆菌拓扑异构酶I的topA基因的P1启动子会以一种依赖于Fis的方式响应氧化应激而被激活。在此我们表明,Fis对topA的调控会随细胞内Fis浓度的变化而变化。因此,当Fis水平较低时,过氧化氢处理会导致topA激活,而在Fis水平较高时,过氧化氢处理会使topA的P1启动子失活。体内二甲基亚砜足迹分析表明,只有在Fis水平较低且受到应激时,topA启动子区域才会发生变化且P1启动子变得活跃。高锰酸钾实验表明,低水平的Fis通过促进开放复合物的形成来激活P1转录,而高水平的这种蛋白质则会关闭启动子。DNA酶I足迹分析表明,Fis在八个具有不同亲和力的位点结合topA的启动子区域。一个低亲和力位点与RNA聚合酶的-10、-35六聚体重叠。我们提出,在响应氧化应激时,当Fis水平较低时,它会以高亲和力位点结合topA的启动子区域,从而促进RNA聚合酶募集到P1启动子,而在Fis水平较高时,Fis也会占据低亲和力位点,从而阻止RNA聚合酶的结合。我们的结果表明,氧化应激反应会随着生长阶段和营养环境的变化而变化。

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