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异聚离子通道亚基编码mRNA的共翻译缔合。

Cotranslational association of mRNA encoding subunits of heteromeric ion channels.

作者信息

Liu Fang, Jones David K, de Lange Willem J, Robertson Gail A

机构信息

Department of Neuroscience, Wisconsin Institutes of Medical Research, University of Wisconsin School of Medicine and Public Health, Madison, WI 53705;

Department of Pediatrics, Wisconsin Institutes of Medical Research, University of Wisconsin School of Medicine and Public Health, Madison, WI 53705;

出版信息

Proc Natl Acad Sci U S A. 2016 Apr 26;113(17):4859-64. doi: 10.1073/pnas.1521577113. Epub 2016 Apr 12.

Abstract

Oligomers of homomeric voltage-gated potassium channels associate early in biogenesis as the nascent proteins emerge from the polysome. Less is known about how proteins emerging from different polysomes associate to form hetero-oligomeric channels. Here, we report that alternate mRNA transcripts encoding human ether-à-go-go-related gene (hERG) 1a and 1b subunits, which assemble to produce ion channels mediating cardiac repolarization, are physically associated during translation. We show that shRNA specifically targeting either hERG 1a or 1b transcripts reduced levels of both transcripts, but only when they were coexpressed heterologously. Both transcripts could be copurified with an Ab against the nascent hERG 1a N terminus. This interaction occurred even when translation of 1b was prevented, indicating the transcripts associate independent of their encoded proteins. The association was also demonstrated in cardiomyocytes, where levels of both hERG transcripts were reduced by either 1a or 1b shRNA, but native KCNE1 and ryanodine receptor 2 (RYR2) transcripts were unaffected. Changes in protein levels and membrane currents mirrored changes in transcript levels, indicating the targeted transcripts were undergoing translation. The physical association of transcripts encoding different subunits provides the spatial proximity required for nascent proteins to interact during biogenesis, and may represent a general mechanism facilitating assembly of heteromeric protein complexes involved in a range of biological processes.

摘要

同型电压门控钾通道的寡聚体在生物合成早期就会随着新生蛋白质从多核糖体中出现而缔合。关于来自不同多核糖体的蛋白质如何缔合形成异源寡聚体通道,人们了解得较少。在此,我们报告称,编码人类去极化相关基因(hERG)1a和1b亚基的交替mRNA转录本在翻译过程中会发生物理缔合,这两个亚基组装形成介导心脏复极化的离子通道。我们发现,特异性靶向hERG 1a或1b转录本的短发夹RNA(shRNA)会降低这两种转录本的水平,但只有在它们异源共表达时才会出现这种情况。这两种转录本都可以用针对新生hERG 1a N端的抗体进行共纯化。即使阻止1b的翻译,这种相互作用仍然会发生,这表明转录本的缔合独立于其编码的蛋白质。在心肌细胞中也证实了这种缔合,其中hERG 1a或1b的shRNA会降低两种hERG转录本的水平,但天然的KCNE1和兰尼碱受体2(RYR2)转录本不受影响。蛋白质水平和膜电流的变化反映了转录本水平的变化,表明靶向的转录本正在进行翻译。编码不同亚基的转录本之间的物理缔合为新生蛋白质在生物合成过程中相互作用提供了所需的空间接近性,并且可能代表了一种促进参与一系列生物过程的异源蛋白质复合物组装的普遍机制。

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