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8个核苷酸长的RNA:DNA杂交体是RNA聚合酶II延伸复合物的主要稳定性决定因素。

The 8-nucleotide-long RNA:DNA hybrid is a primary stability determinant of the RNA polymerase II elongation complex.

作者信息

Kireeva M L, Komissarova N, Waugh D S, Kashlev M

机构信息

Advanced BioScience Laboratories, Inc.-Basic Research Program, NCI-Frederick Cancer Research and Development Center, National Institutes of Health, Frederick, Maryland 21702-1201, USA.

出版信息

J Biol Chem. 2000 Mar 3;275(9):6530-6. doi: 10.1074/jbc.275.9.6530.

Abstract

The sliding clamp model of transcription processivity, based on extensive studies of Escherichia coli RNA polymerase, suggests that formation of a stable elongation complex requires two distinct nucleic acid components: an 8-9-nt transcript-template hybrid, and a DNA duplex immediately downstream from the hybrid. Here, we address the minimal composition of the processive elongation complex in the eukaryotes by developing a method for promoter-independent assembly of functional elongation complex of S. cerevisiae RNA polymerase II from synthetic DNA and RNA oligonucleotides. We show that only one of the nucleic acid components, the 8-nt RNA:DNA hybrid, is necessary for the formation of a stable elongation complex with RNA polymerase II. The double-strand DNA upstream and downstream of the hybrid does not affect stability of the elongation complex. This finding reveals a significant difference in processivity determinants of RNA polymerase II and E. coli RNA polymerase. In addition, using the imperfect RNA:DNA hybrid disturbed by the mismatches in the RNA, we show that nontemplate DNA strand may reduce the elongation complex stability via the reduction of the RNA:DNA hybrid length. The structure of a "minimal stable" elongation complex suggests a key role of the RNA:DNA hybrid in RNA polymerase II processivity.

摘要

基于对大肠杆菌RNA聚合酶的大量研究,转录持续性的滑动夹模型表明,稳定延伸复合物的形成需要两种不同的核酸成分:一个8 - 9个核苷酸的转录本-模板杂交体,以及杂交体下游紧邻的DNA双链。在这里,我们通过开发一种从合成DNA和RNA寡核苷酸中独立于启动子组装酿酒酵母RNA聚合酶II功能性延伸复合物的方法,来研究真核生物中持续性延伸复合物的最小组成。我们表明,对于与RNA聚合酶II形成稳定延伸复合物而言,核酸成分中只有一个8个核苷酸的RNA:DNA杂交体是必需的。杂交体上下游的双链DNA并不影响延伸复合物的稳定性。这一发现揭示了RNA聚合酶II和大肠杆菌RNA聚合酶在持续性决定因素上的显著差异。此外,使用受RNA中错配干扰的不完美RNA:DNA杂交体,我们表明非模板DNA链可能通过缩短RNA:DNA杂交体长度来降低延伸复合物的稳定性。“最小稳定”延伸复合物的结构表明RNA:DNA杂交体在RNA聚合酶II持续性中起关键作用。

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