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细胞应激诱导的切割 tRNA 片段的全基因组鉴定和定量分析。

Genome-wide identification and quantitative analysis of cleaved tRNA fragments induced by cellular stress.

机构信息

Department of Nutrition, Case Western Reserve University, Cleveland, Ohio 44106, USA.

出版信息

J Biol Chem. 2012 Dec 14;287(51):42708-25. doi: 10.1074/jbc.M112.371799. Epub 2012 Oct 19.

Abstract

Certain stress conditions can induce cleavage of tRNAs around the anticodon loop via the use of the ribonuclease angiogenin. The cellular factors that regulate tRNA cleavage are not well known. In this study we used normal and eIF2α phosphorylation-deficient mouse embryonic fibroblasts and applied a microarray-based methodology to identify and compare tRNA cleavage patterns in response to hypertonic stress, oxidative stress (arsenite), and treatment with recombinant angiogenin. In all three scenarios mouse embryonic fibroblasts deficient in eIF2α phosphorylation showed a higher accumulation of tRNA fragments including those derived from initiator-tRNA(Met). We have shown that tRNA cleavage is regulated by the availability of angiogenin, its substrate (tRNA), the levels of the angiogenin inhibitor RNH1, and the rates of protein synthesis. These conclusions are supported by the following findings: (i) exogenous treatment with angiogenin or knockdown of RNH1 increased tRNA cleavage; (ii) tRNA fragment accumulation was higher during oxidative stress than hypertonic stress, in agreement with a dramatic decrease of RNH1 levels during oxidative stress; and (iii) a positive correlation was observed between angiogenin-mediated tRNA cleavage and global protein synthesis rates. Identification of the stress-specific tRNA cleavage mechanisms and patterns will provide insights into the role of tRNA fragments in signaling pathways and stress-related disorders.

摘要

某些应激条件可以通过使用核糖核酸酶血管生成素诱导反密码环周围的 tRNA 切割。调节 tRNA 切割的细胞因子尚不清楚。在这项研究中,我们使用正常和 eIF2α 磷酸化缺陷型小鼠胚胎成纤维细胞,并应用基于微阵列的方法来鉴定和比较响应高渗应激、氧化应激(亚砷酸盐)和重组血管生成素处理的 tRNA 切割模式。在所有三种情况下,eIF2α 磷酸化缺陷的小鼠胚胎成纤维细胞显示出更高的 tRNA 片段积累,包括来自起始 tRNA(Met)的片段。我们已经表明,tRNA 切割受血管生成素、其底物 (tRNA)、血管生成素抑制剂 RNH1 的水平和蛋白质合成速率的可用性调节。这些结论得到了以下发现的支持:(i) 外源性给予血管生成素或敲低 RNH1 增加了 tRNA 切割;(ii) 氧化应激期间的 tRNA 片段积累高于高渗应激,与氧化应激期间 RNH1 水平的急剧下降一致;和 (iii) 观察到血管生成素介导的 tRNA 切割与全局蛋白质合成速率之间存在正相关。鉴定应激特异性 tRNA 切割机制和模式将深入了解 tRNA 片段在信号通路和应激相关疾病中的作用。

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