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Mapping of the OxyR protein contact site in the C-terminal region of RNA polymerase alpha subunit.

机译:RNA聚合酶α亚基的C端区域中的OxyR蛋白接触位点的图谱。

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摘要

The Escherichia coli OxyR protein requires the C-terminal contact site I region of the RNA polymerase alpha subunit for cooperative interaction with and transcription activation at OxyR-dependent promoters, suggesting direct protein-protein contact between OxyR and the C-terminal region of the alpha subunit. To determine the precise location of the OxyR protein contact site(s) in this region, we carried out mutational analysis of the 3' half of E. coli rpoA, the gene encoding the alpha subunit of RNA polymerase. We isolated a number of rpoA mutants defective in oxyR-dependent transcription activation at the E. coli katG promoter. Nucleotide sequence analysis of the rpoA gene from these mutants revealed that the mutations showing clear phenotypes are all clustered at two narrow regions (amino acid residues 265 to 269 and 293 to 300) within the C terminus of the alpha subunit. Reconstituted RNA polymerases containing the mutant alpha subunits were unable to respond to transcription activation in vitro at the katG, ahpC, and oxyX promoters by OxyR. These results suggest that these two regions comprise the contact surfaces on the alpha subunit for OxyR.
机译:大肠杆菌OxyR蛋白需要​​RNA聚合酶α亚基的C末端接触位点I区与OxyR依赖性启动子协同相互作用并在其上激活转录,这表明OxyR与α的C末端区之间存在直接的蛋白质接触亚基。为了确定该区域中OxyR蛋白接触位点的精确位置,我们对大肠杆菌rpoA的3'半部分进行了突变分析,该基因编码RNA聚合酶的α亚基。我们在大肠杆菌katG启动子上分离了许多oxyR依赖性转录激活缺陷的rpoA突变体。对来自这些突变体的rpoA基因的核苷酸序列分析表明,显示清晰表型的突变都聚集在α亚基C端的两个狭窄区域(氨基酸残基265至269和293至300)。含有突变体α亚基的重组RNA聚合酶无法在体外响应OxyR在katG,ahpC和oxyX启动子上的转录激活。这些结果表明,这两个区域包括OxyR的α亚基上的接触表面。

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