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在核糖体在信使核糖核酸(mRNA)上发生滑动期间,对转运核糖核酸(tRNA)结构、核糖体蛋白L9以及噬菌体T4基因60的通读信号所起作用的分析。

Analysis of the roles of tRNA structure, ribosomal protein L9, and the bacteriophage T4 gene 60 bypassing signals during ribosome slippage on mRNA.

作者信息

Herr A J, Nelson C C, Wills N M, Gesteland R F, Atkins J F

机构信息

Department of Human Genetics, University of Utah, 2030 E 15N, RM 7410, Salt Lake City, UT, 84112-5330, USA.

出版信息

J Mol Biol. 2001 Jun 22;309(5):1029-48. doi: 10.1006/jmbi.2001.4717.

DOI:10.1006/jmbi.2001.4717
PMID:11399077
Abstract

A 50-nucleotide coding gap divides bacteriophage T4 gene 60 into two open reading frames. In response to cis-acting stimulatory signals encrypted in the mRNA, the anticodon of the ribosome-bound peptidyl tRNA dissociates from a GGA codon at the end of the first open reading frame and pairs with a GGA codon 47 nucleotides downstream just before the second open reading frame. Mutations affecting ribosomal protein L9 or tRNA(Gly)(2), the tRNA that decodes GGA, alter the efficiency of bypassing. To understand the mechanism of ribosome slippage, this work analyzes the influence of these bypassing signals and mutant translational components on -1 frameshifting at G GGA and hopping over a stop codon immediately flanked by two GGA glycine codons (stop-hopping). Mutant variants of tRNA(Gly)(2) that impair bypassing mediate stop-hopping with unexpected landing specificities, suggesting that these variants are defective in ribosomal P-site codon-anticodon pairing. In a direct competition between -1 frameshifting and stop-hopping, the absence of L9 promotes stop-hopping at the expense of -1 frameshifting without substantially impairing the ability of mutant tRNA(Gly)(2) variants to re-pair with the mRNA by sub-optimal pairing. These observations suggest that L9 defects may stimulate ribosome slippage by enhancing mRNA movement through the ribosome rather than by inducing an extended pause in translation or by destabilizing P-site pairing. Two of the bypassing signals, a cis-acting nascent peptide encoded by the first open reading frame and a stemloop signal located in the 5' portion of the coding gap, stimulate peptidyl-tRNA slippage independently of the rest of the gene 60 context. Evidence is presented suggesting that the nascent peptide signal may stimulate bypassing by destabilizing P-site pairing.

摘要

一个50个核苷酸的编码间隔将噬菌体T4基因60分成两个开放阅读框。响应于mRNA中加密的顺式作用刺激信号,核糖体结合的肽基tRNA的反密码子从第一个开放阅读框末端的GGA密码子解离,并与第二个开放阅读框之前下游47个核苷酸处的GGA密码子配对。影响核糖体蛋白L9或tRNA(Gly)(2)(解码GGA的tRNA)的突变会改变跳跃的效率。为了理解核糖体滑移的机制,这项工作分析了这些跳跃信号和突变翻译组件对在G GGA处的-1移码以及跳过紧邻两个GGA甘氨酸密码子的终止密码子(终止跳跃)的影响。损害跳跃的tRNA(Gly)(2)突变变体介导具有意外着陆特异性的终止跳跃,这表明这些变体在核糖体P位点密码子-反密码子配对方面存在缺陷。在-1移码和终止跳跃的直接竞争中,L9的缺失以-1移码为代价促进终止跳跃,而不会实质性损害突变tRNA(Gly)(2)变体通过次优配对与mRNA重新配对的能力。这些观察结果表明,L9缺陷可能通过增强mRNA通过核糖体的移动来刺激核糖体滑移,而不是通过诱导翻译中的延长停顿或通过破坏P位点配对来实现。两个跳跃信号,一个由第一个开放阅读框编码的顺式作用新生肽和一个位于编码间隔5'部分的茎环信号,独立于基因60的其余背景刺激肽基-tRNA滑移。有证据表明新生肽信号可能通过破坏P位点配对来刺激跳跃。

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