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特殊的肽基转移RNA分子可以促进翻译移码而不发生滑动。

Special peptidyl-tRNA molecules can promote translational frameshifting without slippage.

作者信息

Vimaladithan A, Farabaugh P J

机构信息

Department of Biological Sciences, University of Maryland, Baltimore 21228.

出版信息

Mol Cell Biol. 1994 Dec;14(12):8107-16. doi: 10.1128/mcb.14.12.8107-8116.1994.

Abstract

Recently we described an unusual programmed +1 frameshift event in yeast retrotransposon Ty3. Frameshifting depends on the presence of peptidyl-tRNA(AlaCGC) on the GCG codon in the ribosomal P site and on a translational pause stimulated by the slowly decoded AGU codon. Frameshifting occurs on the sequence GCG-AGU-U by out-of-frame binding of a valyl-tRNA to GUU without slippage of peptidyl-tRNA(AlaCGC). This mechanism challenges the conventional understanding that frameshift efficiency must correlate with the ability of mRNA-bound tRNA to slip between cognate or near-cognate codons. Though frameshifting does not require slippery tRNAs, it does require special peptidyl-tRNAs. We show that overproducing a second isoacceptor whose anticodon had been changed to CGC eliminated frameshifting; peptidyl-tRNA(AlaCGC) must have a special capacity to induce +1 frameshifting in the adjacent ribosomal A site. In order to identify other special peptidyl-tRNAs, we tested the ability of each of the other 63 codons to replace GCG in the P site. We found no correlation between the ability to stimulate +1 frameshifting and the ability of the cognate tRNA to slip on the mRNA--several codons predicted to slip efficiently do not stimulate frameshifting, while several predicted not to slip do stimulate frameshifting. By inducing a severe translational pause, we identified eight tRNAs capable of inducing measurable +1 frameshifting, only four of which are predicted to slip on the mRNA. We conclude that in Saccharomyces cerevisiae, special peptidyl-tRNAs can induce frameshifting dependent on some characteristic(s) other than the ability to slip on the mRNA.

摘要

最近,我们描述了酵母逆转录转座子Ty3中一种不寻常的程序性+1移码事件。移码取决于核糖体P位点上GCG密码子处肽基-tRNA(AlaCGC)的存在以及由缓慢解码的AGU密码子刺激的翻译暂停。移码发生在序列GCG-AGU-U上,是由于缬氨酰-tRNA与GUU的框外结合,而肽基-tRNA(AlaCGC)没有滑动。这种机制挑战了传统观念,即移码效率必须与mRNA结合的tRNA在同源或近同源密码子之间滑动的能力相关。虽然移码不需要滑动tRNA,但确实需要特殊的肽基-tRNA。我们发现,过量产生第二种反密码子已变为CGC的同功受体消除了移码;肽基-tRNA(AlaCGC)必须具有在相邻核糖体A位点诱导+1移码的特殊能力。为了鉴定其他特殊的肽基-tRNA,我们测试了其他63个密码子中的每一个替换P位点上GCG的能力。我们发现刺激+1移码的能力与同源tRNA在mRNA上滑动的能力之间没有相关性——几个预计能有效滑动的密码子不会刺激移码,而几个预计不会滑动的密码子却会刺激移码。通过诱导严重的翻译暂停,我们鉴定出了八种能够诱导可测量的+1移码的tRNA,其中只有四种预计会在mRNA上滑动。我们得出结论,在酿酒酵母中,特殊的肽基-tRNA可以诱导移码,这种移码依赖于除在mRNA上滑动能力之外的某些特征。

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