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重组嗜热栖热菌RNA聚合酶,一种用于基于结构的转录分析的新工具。

Recombinant Thermus aquaticus RNA polymerase, a new tool for structure-based analysis of transcription.

作者信息

Minakhin L, Nechaev S, Campbell E A, Severinov K

机构信息

Waksman Institute for Microbiology and Department of Genetics, Rutgers, The State University of New Jersey, Piscataway, New Jersey 08854, USA.

出版信息

J Bacteriol. 2001 Jan;183(1):71-6. doi: 10.1128/JB.183.1.71-76.2001.

Abstract

The three-dimensional structure of DNA-dependent RNA polymerase (RNAP) from thermophilic Thermus aquaticus has recently been determined at 3.3 A resolution. Currently, very little is known about T. aquaticus transcription and no genetic system to study T. aquaticus RNAP genes is available. To overcome these limitations, we cloned and overexpressed T. aquaticus RNAP genes in Escherichia coli. Overproduced T. aquaticus RNAP subunits assembled into functional RNAP in vitro and in vivo when coexpressed in E. coli. We used the recombinant T. aquaticus enzyme to demonstrate that transcription initiation, transcription termination, and transcription cleavage assays developed for E. coli RNAP can be adapted to study T. aquaticus transcription. However, T. aquaticus RNAP differs from the prototypical E. coli enzyme in several important ways: it terminates transcription less efficiently, has exceptionally high rate of intrinsic transcript cleavage, and is highly resistant to rifampin. Our results, together with the high-resolution structural information, should now allow a rational analysis of transcription mechanism by mutation.

摘要

嗜热栖热菌(Thermus aquaticus)依赖DNA的RNA聚合酶(RNAP)的三维结构最近已在3.3埃分辨率下确定。目前,关于栖热菌转录的了解非常少,并且没有可用于研究栖热菌RNAP基因的遗传系统。为了克服这些限制,我们在大肠杆菌中克隆并过量表达了栖热菌RNAP基因。当在大肠杆菌中共表达时,过量产生的栖热菌RNAP亚基在体外和体内组装成功能性RNAP。我们使用重组栖热菌酶来证明,为大肠杆菌RNAP开发的转录起始、转录终止和转录切割分析方法可适用于研究栖热菌转录。然而,栖热菌RNAP在几个重要方面与典型的大肠杆菌酶不同:它终止转录的效率较低,具有异常高的内在转录切割速率,并且对利福平具有高度抗性。我们的结果,连同高分辨率结构信息,现在应该能够通过突变对转录机制进行合理分析。

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