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The redox-regulated SoxR protein acts from a single DNA site as a repressor and an allosteric activator.

机译:氧化还原调节的SoxR蛋白从单个DNA位点起阻遏物和变构活化剂的作用。

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摘要

The SoxR protein of Escherichia coli responds to redox signals by activating the transcription of soxS, which encodes another transcription activator that directly stimulates oxidative stress genes. We show here that transcription of the soxR gene, which is positioned head-to-head with soxS in the chromosome, initiates in the intergenic region and is itself repressed by SoxR protein in in vitro transcription experiments. Analysis of single-copy operon fusions to soxR, combined with the results of Northern blotting experiments, verified this regulation and the transcription start site in vivo. The structure of the overlapping promoters is such that the single SoxR-binding site is located in the -10/-35 spacer of the soxS promoter, but just downstream of the -10 element of the soxR promoter. Activated and non-activated SoxR bind this site equally well, exerting nearly constant repression of soxR; activated SoxR simultaneously stimulates the soxS promoter >/=30-fold. The functional soxR promoter depresses soxS transcription when SoxR is not activated and enhances soxS transcription when SoxR is activated, as shown by comparing the expression of soxS'::lacZ fusions with and without the soxR -35 element (induction ratio only approximately 7-fold). SoxR thus represents a highly polar, redox-regulated transcriptional switch that maximizes the change in expression of soxS.
机译:大肠杆菌的SoxR蛋白通过激活soxS的转录来响应氧化还原信号,后者编码另一种直接激活氧化应激基因的转录激活剂。我们在这里显示,在染色体转录中与soxS并排放置的soxR基因的转录起始于基因间区域,并且在体外转录实验中本身被SoxR蛋白抑制。与soxR的单拷贝操纵子融合体的分析,与Northern blotting实验的结果相结合,验证了这种调节和体内转录起始位点。重叠启动子的结构使得单个SoxR结合位点位于soxS启动子的-10 / -35间隔区中,但仅在soxR启动子的-10元件的下游。激活的和未激活的SoxR均能很好地结合该位点,从而几乎持续抑制soxR。激活的SoxR同时刺激soxS启动子> / = 30倍。有功能的soxR启动子在未激活SoxR时抑制soxS转录,并在激活SoxR时增强soxS转录,如比较带有和不带有soxR -35元素的soxS':: lacZ融合蛋白的表达(诱导率仅约7倍) )。因此,SoxR代表了一种高度极性的,氧化还原调节的转录开关,可最大限度地提高soxS表达的变化。

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