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真核生物翻译起始的扫描机制。

The scanning mechanism of eukaryotic translation initiation.

机构信息

Laboratory of Gene Regulation and Development, Eunice Kennedy Shriver National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892; email:

出版信息

Annu Rev Biochem. 2014;83:779-812. doi: 10.1146/annurev-biochem-060713-035802. Epub 2014 Jan 29.

Abstract

In eukaryotes, the translation initiation codon is generally identified by the scanning mechanism, wherein every triplet in the messenger RNA leader is inspected for complementarity to the anticodon of methionyl initiator transfer RNA (Met-tRNAi). Binding of Met-tRNAi to the small (40S) ribosomal subunit, in a ternary complex (TC) with eIF2-GTP, is stimulated by eukaryotic initiation factor 1 (eIF1), eIF1A, eIF3, and eIF5, and the resulting preinitiation complex (PIC) joins the 5' end of mRNA preactivated by eIF4F and poly(A)-binding protein. RNA helicases remove secondary structures that impede ribosome attachment and subsequent scanning. Hydrolysis of eIF2-bound GTP is stimulated by eIF5 in the scanning PIC, but completion of the reaction is impeded at non-AUG triplets. Although eIF1 and eIF1A promote scanning, eIF1 and possibly the C-terminal tail of eIF1A must be displaced from the P decoding site to permit base-pairing between Met-tRNAi and the AUG codon, as well as to allow subsequent phosphate release from eIF2-GDP. A second GTPase, eIF5B, catalyzes the joining of the 60S subunit to produce an 80S initiation complex that is competent for elongation.

摘要

在真核生物中,翻译起始密码子通常通过扫描机制来识别,其中信使 RNA 前导区的每个三联体都被检查是否与甲硫氨酰起始转移 RNA(Met-tRNAi)的反密码子互补。Met-tRNAi 与小(40S)核糖体亚基结合,形成三元复合物(TC)与 eIF2-GTP,受真核起始因子 1(eIF1)、eIF1A、eIF3 和 eIF5 的刺激,生成的起始前复合物(PIC)与 eIF4F 和 poly(A)-结合蛋白预激活的 mRNA 5'端结合。RNA 解旋酶去除阻碍核糖体附着和随后扫描的二级结构。扫描 PIC 中的 eIF5 刺激 eIF2 结合的 GTP 水解,但在非 AUG 三联体处完成反应受到阻碍。虽然 eIF1 和 eIF1A 促进扫描,但 eIF1 和可能是 eIF1A 的 C 末端尾巴必须从 P 解码位点位移,以允许 Met-tRNAi 与 AUG 密码子配对,以及允许随后从 eIF2-GDP 释放磷酸基团。第二种 GTPase,eIF5B,催化 60S 亚基的结合,产生能够进行延伸的 80S 起始复合物。

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