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翻译起始因子 eIF4GII 的多种同工型通过使用不同的启动子、剪接位点和非规范起始密码子生成。

Multiple isoforms of the translation initiation factor eIF4GII are generated via use of alternative promoters, splice sites and a non-canonical initiation codon.

机构信息

Department of Biochemistry, School of Life Sciences, University of Sussex, Falmer, Brighton BN1 9QG, UK.

出版信息

Biochem J. 2012 Nov 15;448(1):1-11. doi: 10.1042/BJ20111765.

DOI:10.1042/BJ20111765
PMID:22909319
Abstract

During the initiation stage of eukaryotic mRNA translation, the eIF4G (eukaryotic initiation factor 4G) proteins act as an aggregation point for recruiting the small ribosomal subunit to an mRNA. We previously used RNAi (RNA interference) to reduce expression of endogenous eIF4GI proteins, resulting in reduced protein synthesis rates and alterations in the morphology of cells. Expression of EIF4G1 cDNAs, encoding different isoforms (f-a) which arise through selection of alternative initiation codons, rescued translation to different extents. Furthermore, overexpression of the eIF4GII paralogue in the eIF4GI-knockdown background was unable to restore translation to the same extent as eIF4GIf/e isoforms, suggesting that translation events governed by this protein are different. In the present study we show that multiple isoforms of eIF4GII exist in mammalian cells, arising from multiple promoters and alternative splicing events, and have identified a non-canonical CUG initiation codon which extends the eIF4GII N-terminus. We further show that the rescue of translation in eIF4GI/eIF4GII double-knockdown cells by our novel isoforms of eIF4GII is as robust as that observed with either eIF4GIf or eIF4GIe, and more than that observed with the original eIF4GII. As the novel eIF4GII sequence diverges from eIF4GI, these data suggest that the eIF4GII N-terminus plays an alternative role in initiation factor assembly.

摘要

在真核生物 mRNA 翻译的起始阶段,eIF4G(真核起始因子 4G)蛋白作为一个聚集点,将小核糖体亚基招募到 mRNA 上。我们之前使用 RNAi(RNA 干扰)来降低内源性 eIF4GI 蛋白的表达,导致蛋白质合成速率降低和细胞形态改变。表达编码不同异构体(f-a)的 EIF4G1 cDNA,这些异构体通过选择不同的起始密码子产生,在不同程度上拯救了翻译。此外,在 eIF4GI 敲低背景下过表达 eIF4GII 同源物,不能像 eIF4GIf/e 异构体那样恢复翻译,这表明该蛋白控制的翻译事件不同。在本研究中,我们表明哺乳动物细胞中存在多种 eIF4GII 异构体,它们由多个启动子和选择性剪接事件产生,并鉴定了一个非典型的 CUG 起始密码子,该密码子延伸了 eIF4GII 的 N 端。我们进一步表明,我们新型的 eIF4GII 异构体在 eIF4GI/eIF4GII 双敲低细胞中对翻译的拯救作用与 eIF4GIf 或 eIF4GIe 观察到的一样强大,并且比原始 eIF4GII 观察到的更强。由于新型 eIF4GII 序列与 eIF4GI 不同,这些数据表明 eIF4GII N 端在起始因子组装中发挥替代作用。

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Multiple isoforms of the translation initiation factor eIF4GII are generated via use of alternative promoters, splice sites and a non-canonical initiation codon.翻译起始因子 eIF4GII 的多种同工型通过使用不同的启动子、剪接位点和非规范起始密码子生成。
Biochem J. 2012 Nov 15;448(1):1-11. doi: 10.1042/BJ20111765.
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Generation of multiple isoforms of eukaryotic translation initiation factor 4GI by use of alternate translation initiation codons.通过使用可变翻译起始密码子产生真核生物翻译起始因子4GI的多种同工型。
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