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σ因子和σ⁷⁰ RNA聚合酶全酶转录效率差异参与大肠杆菌osmE启动子生长阶段调控

Involvement of differential efficiency of transcription by esigmas and esigma70 RNA polymerase holoenzymes in growth phase regulation of the Escherichia coli osmE promoter.

作者信息

Bordes P, Repoila F, Kolb A, Gutierrez C

机构信息

Laboratoire de Microbiologie et Génétique Moléculaire, UPR 9007 CNRS, 118 Route de Narbonne, F-31062 Toulouse Cedex, France.

出版信息

Mol Microbiol. 2000 Feb;35(4):845-53. doi: 10.1046/j.1365-2958.2000.01758.x.

DOI:10.1046/j.1365-2958.2000.01758.x
PMID:10692161
Abstract

Transcription of the gene osmE of Escherichia coli is inducible by elevated osmotic pressure and during the decelerating phase of growth. osmE expression is directed by a single promoter, osmEp. Decelerating phase induction of osmEp is dependent on the sigmas (RpoS) factor, whereas its osmotic induction is independent of sigmas. Purified Esigmas and Esigma70 were both able to transcribe osmEp in vitro on supercoiled templates. In the presence of rpoD800, a mutation resulting in a thermosensitive sigma70 factor, a shift to non-permissive temperature abolished induction of osmEp after an osmotic shock during exponential phase, but did not affect the decelerating phase induction. Point mutations affecting osmEp activity were isolated. Down-promoter mutations decreased transcription in both the presence and the absence of sigmas, indicating that the two forms of RNA polymerase holoenzyme recognize very similar sequence determinants on the osmE promoter. Three up-promoter mutations brought osmEp closer to the consensus of Esigma70-dependent promoters. The two variant promoters exhibiting the highest efficiency became essentially independent of sigmas in vivo. Our data suggest that Esigmas transcribes wild-type osmEp with a higher efficiency than Esigma70. A model in which an intrinsic differential recognition contributes to growth phase-dependent regulation is proposed. Generalization of this model to other sigmas-dependent promoters is discussed.

摘要

大肠杆菌基因osmE的转录可由渗透压升高及生长减速期诱导。osmE的表达由单一启动子osmEp指导。osmEp在生长减速期的诱导依赖于σ因子(RpoS),而其渗透压诱导则不依赖于σ因子。纯化的EσS和Eσ70均能在体外超螺旋模板上转录osmEp。在rpoD800存在的情况下,rpoD800是一种导致温度敏感型σ70因子的突变,在指数生长期经渗透压休克后,转移至非允许温度会消除osmEp的诱导,但不影响生长减速期的诱导。分离出了影响osmEp活性的点突变。启动子下游突变在有和没有σ因子的情况下均降低了转录,这表明两种形式的RNA聚合酶全酶在osmE启动子上识别非常相似的序列决定簇。三个启动子上游突变使osmEp更接近Eσ70依赖型启动子的共有序列。在体内,两个效率最高的变体启动子基本不依赖于σ因子。我们的数据表明,EσS转录野生型osmEp的效率高于Eσ70。提出了一个内在差异识别有助于生长阶段依赖性调控的模型。讨论了将该模型推广到其他σ因子依赖型启动子的情况。

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