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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。

Generation of multiple isoforms of eukaryotic translation initiation factor 4GI by use of alternate translation initiation codons.

作者信息

Byrd Marshall P, Zamora Miguel, Lloyd Richard E

机构信息

Department of Molecular Virology and Microbiology, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

Mol Cell Biol. 2002 Jul;22(13):4499-511. doi: 10.1128/MCB.22.13.4499-4511.2002.

Abstract

Eukaryotic translation initiation factor 4GI (eIF4GI) is an essential protein that is the target for translational regulation in many cellular processes and viral systems. It has been shown to function in both cap-dependent and cap-independent translation initiation by recruiting the 40S ribosomal subunit to the mRNA cap structure or internal ribosome entry site (IRES) element, respectively. Interestingly eIF4GI mRNA itself has been reported to contain an IRES element in its 5' end that facilitates eIF4GI protein synthesis via a cap-independent mechanism. In HeLa cells, eIF4GI exists as several isoforms that differ in their migration in sodium dodecyl sulfate (SDS) gels; however, the nature of these isoforms was unclear. Here, we report a new cDNA clone for eIF4GI that extends the 5' sequence 340 nucleotides beyond the previously published sequence. The new extended sequence of eIF4GI is located on chromosome 3, within two additional exons immediately upstream of the previously published eIF4GI sequence. When mRNA transcribed from this cDNA clone was translated in vitro, five eIF4GI polypeptides were generated that comigrated in SDS-polyacrylamide gels with the five isoforms of native eIF4GI. Furthermore, translation of eIF4GI-enhanced green fluorescent protein fusion constructs in vitro or in vivo generated five isoforms of fusion polypeptides, suggesting that multiple isoforms of eIF4GI are generated by alternative translation initiation in vitro and in vivo. Mutation of two of the five in-frame AUG residues in the eIF4GI cDNA sequence resulted in loss of corresponding polypeptides after translation in vitro, confirming alternate use of AUGs as the source of the multiple polypeptides. The 5' untranslated region of eIF4GI mRNA also contains an out-of-frame open reading frame (ORF) that may down-regulate expression of eIF4GI. Further, data are presented to suggest that a proposed IRES embedded in the eIF4GI ORF is able to catalyze synthesis of multiple eIF4GI isoforms as well. Our data suggest that expression of the eIF4GI isoforms is partly controlled by a complex translation strategy involving both cap-dependent and cap-independent mechanisms.

摘要

真核生物翻译起始因子4GI(eIF4GI)是一种必需蛋白,在许多细胞过程和病毒系统中是翻译调控的靶点。研究表明,它分别通过将40S核糖体亚基募集到mRNA帽结构或内部核糖体进入位点(IRES)元件,在依赖帽和不依赖帽的翻译起始中发挥作用。有趣的是,据报道eIF4GI mRNA本身在其5'端含有一个IRES元件,可通过不依赖帽的机制促进eIF4GI蛋白的合成。在HeLa细胞中,eIF4GI以几种同工型存在,它们在十二烷基硫酸钠(SDS)凝胶中的迁移情况不同;然而,这些同工型的性质尚不清楚。在这里,我们报道了一个新的eIF4GI cDNA克隆,其5'序列比先前发表的序列延伸了340个核苷酸。eIF4GI的新延伸序列位于3号染色体上,在先前发表的eIF4GI序列上游的另外两个外显子内。当从这个cDNA克隆转录的mRNA在体外进行翻译时,产生了五种eIF4GI多肽,它们在SDS-聚丙烯酰胺凝胶中的迁移情况与天然eIF4GI的五种同工型相同。此外,eIF4GI-增强型绿色荧光蛋白融合构建体在体外或体内的翻译产生了五种融合多肽同工型,这表明eIF4GI的多种同工型是通过体外和体内的可变翻译起始产生的。eIF4GI cDNA序列中五个读框内AUG残基中的两个发生突变,导致体外翻译后相应多肽缺失,证实了AUG作为多种多肽来源的交替使用。eIF4GI mRNA的5'非翻译区还包含一个移码开放阅读框(ORF),可能会下调eIF4GI的表达。此外,有数据表明,嵌入eIF4GI ORF中的一个假定IRES也能够催化多种eIF4GI同工型的合成。我们的数据表明,eIF4GI同工型的表达部分受一种复杂的翻译策略控制,该策略涉及依赖帽和不依赖帽的机制。

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