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从紫色非硫细菌球形红杆菌中分离出的RNA聚合酶全酶的转录特性。

Transcription properties of RNA polymerase holoenzymes isolated from the purple nonsulfur bacterium Rhodobacter sphaeroides.

作者信息

Karls R K, Jin D J, Donohue T J

机构信息

Department of Bacteriology, University of Wisconsin-Madison 53706.

出版信息

J Bacteriol. 1993 Dec;175(23):7629-38. doi: 10.1128/jb.175.23.7629-7638.1993.

Abstract

We have been characterizing RNA polymerase holoenzymes from Rhodobacter sphaeroides. RNA polymerase purified from R. sphaeroides transcribed from promoters recognized by Escherichia coli E sigma 32 or E sigma 70 holoenzyme. Antisera to E. coli sigma 32 or sigma 70 indicated that related polypeptides of approximately 37 kDa (sigma 37) and 93 kDa (sigma 93), respectively, are present in this preparation. Transcription of sigma 32-dependent promoters was observed in a further fractionated R. sphaeroides holoenzyme containing the sigma 37 polypeptide, while a preparation enriched in sigma 93 transcribed sigma 70-dependent promoters. To demonstrate further that the sigma 93 polypeptide functions like E. coli sigma 70, we obtained an R. sphaeroides E sigma 93 holoenzyme capable of transcription from sigma 70-dependent promoters by combining sigma 93 with (i) an E sigma 37 fraction with diminished sigma 93 polypeptide content or (ii) E. coli core RNA polymerase. The generation of analogous DNase I footprints on the lacUV5 promoter by R. sphaeroides E sigma 93 and by E. coli E sigma 70 suggests that the overall structures of these two holoenzymes are similar. However, some differences in promoter specificity between R. sphaeroides E sigma 93 and E. coli E sigma 70 exist because transcription of an R. sphaeroides rRNA promoter was detected only with E sigma 93.

摘要

我们一直在对球形红细菌的RNA聚合酶全酶进行特性分析。从球形红细菌中纯化得到的RNA聚合酶可转录由大肠杆菌E σ32或E σ70全酶识别的启动子。针对大肠杆菌σ32或σ70的抗血清表明,该制剂中分别存在约37 kDa(σ37)和93 kDa(σ93)的相关多肽。在含有σ37多肽的进一步分级分离的球形红细菌全酶中观察到了σ32依赖性启动子的转录,而富含σ93的制剂转录了σ70依赖性启动子。为了进一步证明σ93多肽的功能类似于大肠杆菌的σ70,我们通过将σ93与(i)σ93多肽含量降低的E σ37组分或(ii)大肠杆菌核心RNA聚合酶结合,获得了一种能够从σ70依赖性启动子转录的球形红细菌E σ93全酶。球形红细菌E σ93和大肠杆菌E σ70在lacUV5启动子上产生类似的DNase I足迹,这表明这两种全酶的整体结构相似。然而,球形红细菌E σ93和大肠杆菌E σ70之间在启动子特异性上存在一些差异,因为仅用E σ93检测到了球形红细菌rRNA启动子的转录。

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