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在核糖体回收受损的酵母细胞中重新编程翻译有利于翻译效率高的短 mRNA。

Reprogramming of translation in yeast cells impaired for ribosome recycling favors short, efficiently translated mRNAs.

机构信息

Division of Molecular and Cellular Biology, Eunice Kennedy Shriver National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, United States.

Laboratory of Biochemistry and Genetics, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, United States.

出版信息

Elife. 2021 Mar 25;10:e64283. doi: 10.7554/eLife.64283.

Abstract

In eukaryotes, 43S preinitiation complex (PIC) formation is a rate-determining step of translation. Ribosome recycling following translation termination produces free 40S subunits for re-assembly of 43S PICs. Yeast mutants lacking orthologs of mammalian eIF2D (Tma64), and either MCT-1 (Tma20) or DENR (Tma22), are broadly impaired for 40S recycling; however, it was unknown whether this defect alters the translational efficiencies (TEs) of particular mRNAs. Here, we conducted ribosome profiling of a yeast double mutant and observed a marked reprogramming of translation, wherein the TEs of the most efficiently translated ('strong') mRNAs increase, while those of 'weak' mRNAs generally decline. Remarkably, similar reprogramming was seen on reducing 43S PIC assembly by inducing phosphorylation of eIF2α or by decreasing total 40S subunit levels by depleting Rps26. Our findings suggest that strong mRNAs outcompete weak mRNAs in response to 43S PIC limitation achieved in various ways, in accordance with previous mathematical modeling.

摘要

在真核生物中,43S 起始复合物(PIC)的形成是翻译的限速步骤。翻译终止后核糖体的回收产生了游离的 40S 亚基,用于重新组装 43S PIC。缺乏哺乳动物 eIF2D(Tma64)同源物的酵母突变体,以及 MCT-1(Tma20)或 DENR(Tma22),在 40S 回收方面普遍受到广泛影响;然而,尚不清楚这种缺陷是否会改变特定 mRNA 的翻译效率(TE)。在这里,我们对酵母双突变体进行了核糖体谱分析,观察到翻译的明显重编程,其中翻译效率最高的(“强”)mRNA 的 TE 增加,而“弱”mRNA 的 TE 通常下降。值得注意的是,通过诱导 eIF2α 磷酸化或通过耗尽 Rps26 降低总 40S 亚基水平来减少 43S PIC 组装,也观察到类似的重编程。我们的发现表明,与弱 mRNA 相比,强 mRNA 在以各种方式实现的 43S PIC 限制下具有竞争优势,这与之前的数学模型一致。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ecb6/7993997/be95106d0932/elife-64283-fig1.jpg

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