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RNA结合蛋白在RNA稳定性调控中作用的系统分析

Systematic analysis of the role of RNA-binding proteins in the regulation of RNA stability.

作者信息

Hasan Ayesha, Cotobal Cristina, Duncan Caia D S, Mata Juan

机构信息

Department of Biochemistry, University of Cambridge, Cambridge, United Kingdom.

出版信息

PLoS Genet. 2014 Nov 6;10(11):e1004684. doi: 10.1371/journal.pgen.1004684. eCollection 2014 Nov.

Abstract

mRNA half-lives are transcript-specific and vary over a range of more than 100-fold in eukaryotic cells. mRNA stabilities can be regulated by sequence-specific RNA-binding proteins (RBPs), which bind to regulatory sequence elements and modulate the interaction of the mRNA with the cellular RNA degradation machinery. However, it is unclear if this kind of regulation is sufficient to explain the large range of mRNA stabilities. To address this question, we examined the transcriptome of 74 Schizosaccharomyces pombe strains carrying deletions in non-essential genes encoding predicted RBPs (86% of all such genes). We identified 25 strains that displayed changes in the levels of between 4 and 104 mRNAs. The putative targets of these RBPs formed biologically coherent groups, defining regulons involved in cell separation, ribosome biogenesis, meiotic progression, stress responses and mitochondrial function. Moreover, mRNAs in these groups were enriched in specific sequence motifs in their coding sequences and untranslated regions, suggesting that they are coregulated at the posttranscriptional level. We performed genome-wide RNA stability measurements for several RBP mutants, and confirmed that the altered mRNA levels were caused by changes in their stabilities. Although RBPs regulate the decay rates of multiple regulons, only 16% of all S. pombe mRNAs were affected in any of the 74 deletion strains. This suggests that other players or mechanisms are required to generate the observed range of RNA half-lives of a eukaryotic transcriptome.

摘要

信使核糖核酸(mRNA)的半衰期具有转录特异性,在真核细胞中其变化范围超过100倍。mRNA的稳定性可由序列特异性RNA结合蛋白(RBP)调控,这些蛋白与调控序列元件结合,并调节mRNA与细胞RNA降解机制的相互作用。然而,这种调控是否足以解释mRNA稳定性的大范围变化尚不清楚。为解决这个问题,我们检测了74株粟酒裂殖酵母的转录组,这些菌株在编码预测RBP的非必需基因(所有此类基因的86%)中存在缺失。我们鉴定出25株菌株,其4至104种mRNA的水平发生了变化。这些RBP的推定靶标形成了生物学上连贯的组,定义了参与细胞分裂、核糖体生物合成、减数分裂进程、应激反应和线粒体功能的调控子。此外,这些组中的mRNA在其编码序列和非翻译区富含特定的序列基序,这表明它们在转录后水平受到共调控。我们对几个RBP突变体进行了全基因组RNA稳定性测量,并证实mRNA水平的改变是由其稳定性变化引起的。尽管RBP调节多个调控子的降解速率,但在74个缺失菌株中的任何一个中,只有16%的粟酒裂殖酵母mRNA受到影响。这表明需要其他因素或机制来产生真核转录组中观察到的RNA半衰期范围。

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