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Mof2/Sui1蛋白是翻译准确性的一般监测器。

The Mof2/Sui1 protein is a general monitor of translational accuracy.

作者信息

Cui Y, Dinman J D, Kinzy T G, Peltz S W

机构信息

Department of Molecular Genetics and Microbiology, Robert Wood Johnson Medical School, UMDNJ, Piscataway, New Jersey 08854, USA.

出版信息

Mol Cell Biol. 1998 Mar;18(3):1506-16. doi: 10.1128/MCB.18.3.1506.

Abstract

Although it is essential for protein synthesis to be highly accurate, a number of cases of directed ribosomal frameshifting have been reported in RNA viruses, as well as in procaryotic and eucaryotic genes. Changes in the efficiency of ribosomal frameshifting can have major effects on the ability of cells to propagate viruses which use this mechanism. Furthermore, studies of this process can illuminate the mechanisms involved in the maintenance of the normal translation reading frame. The yeast Saccharomyces cerevisiae killer virus system uses programmed -1 ribosomal frameshifting to synthesize its gene products. Strains harboring the mof2-1 allele demonstrated a fivefold increase in frameshifting and prevented killer virus propagation. In this report, we present the results of the cloning and characterization of the wild-type MOF2 gene. mof2-1 is a novel allele of SUI1, a gene previously shown to play a role in translation initiation start site selection. Strains harboring the mof2-1 allele demonstrated a mutant start site selection phenotype and increased efficiency of programmed -1 ribosomal frameshifting and conferred paromomycin sensitivity. The increased frameshifting observed in vivo was reproduced in extracts prepared from mof2-1 cells. Addition of purified wild-type Mof2p/Sui1p reduced frameshifting efficiencies to wild-type levels. Expression of the human SUI1 homolog in yeast corrects all of the mof2-1 phenotypes, demonstrating that the function of this protein is conserved throughout evolution. Taken together, these results suggest that Mof2p/Sui1p functions as a general modulator of accuracy at both the initiation and elongation phases of translation.

摘要

尽管蛋白质合成高度准确至关重要,但在RNA病毒以及原核和真核基因中已报道了许多定向核糖体移码的情况。核糖体移码效率的变化可能对利用这种机制的病毒在细胞中的传播能力产生重大影响。此外,对这一过程的研究可以阐明维持正常翻译阅读框所涉及的机制。酵母酿酒酵母杀伤病毒系统利用程序性-1核糖体移码来合成其基因产物。携带mof2-1等位基因的菌株显示移码增加了五倍,并阻止了杀伤病毒的传播。在本报告中,我们展示了野生型MOF2基因的克隆和表征结果。mof2-1是SUI1的一个新等位基因,SUI1基因先前已被证明在翻译起始位点选择中起作用。携带mof2-1等位基因的菌株表现出突变的起始位点选择表型,程序性-1核糖体移码效率增加,并赋予巴龙霉素敏感性。在体内观察到的移码增加在从mof2-1细胞制备的提取物中重现。添加纯化的野生型Mof2p/Sui1p可将移码效率降低到野生型水平。人SUI1同源物在酵母中的表达纠正了所有mof2-1表型,表明该蛋白质的功能在整个进化过程中是保守的。综上所述,这些结果表明Mof2p/Sui1p在翻译的起始和延伸阶段均作为准确性的一般调节剂发挥作用。

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