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首页> 外文期刊>Molecular Systems Biology >Alternative polyadenylation diversifies post‐transcriptional regulation by selective RNA–protein interactions
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Alternative polyadenylation diversifies post‐transcriptional regulation by selective RNA–protein interactions

机译:选择性的聚腺苷酸化通过选择性的RNA-蛋白质相互作用使转录后调控多样化

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AbstractRecent research has uncovered extensive variability in the boundaries of transcript isoforms, yet the functional consequences of this variation remain largely unexplored. Here, we systematically discriminate between the molecular phenotypes of overlapping coding and non-coding transcriptional events from each genic locus using a novel genome-wide, nucleotide-resolution technique to quantify the half-lives of 3′ transcript isoforms in yeast. Our results reveal widespread differences in stability among isoforms for hundreds of genes in a single condition, and that variation of even a single nucleotide in the 3′ untranslated region (UTR) can affect transcript stability. While previous instances of negative associations between 3′ UTR length and transcript stability have been reported, here, we find that shorter isoforms are not necessarily more stable. We demonstrate the role of RNA-protein interactions in conditioning isoform-specific stability, showing that PUF3 binds and destabilizes specific polyadenylation isoforms. Our findings indicate that although the functional elements of a gene are encoded in DNA sequence, the selective incorporation of these elements into RNA through transcript boundary variation allows a single gene to have diverse functional consequences.SynopsisA single gene can give rise to many isoforms via alternative polyadenylation. This study demonstrates that isoforms of each gene can have different molecular phenotypes like RNA stability and interaction with proteins, diversifying the functional potential of the genome.Divergent post-transcriptional fates of 3′ transcript isoforms are revealed at a genome-wide level.New techniques are presented that accurately measure isoform-specific stability and protein binding, thus demonstrating widespread variation in both.Even variations of a few nucleotides are associated with variations in transcript stability.Transcript binding to PUF3 and subsequent destabilization occurs in an isoform-specific manner.
机译:摘要最近的研究发现转录本同工型的边界存在广泛的变异性,但这种变异的功能性后果仍未得到充分探索。在这里,我们使用新型的全基因组核苷酸分辨率技术来量化酵母中3'转录本同工型的半衰期,从而系统地区分了来自每个基因位点的重叠编码和非编码转录事件的分子表型。我们的结果揭示了在单一条件下数百个基因的同工型之间稳定性的广泛差异,并且3'非翻译区(UTR)中甚至单个核苷酸的变异也会影响转录本的稳定性。虽然以前报道了3'UTR长度和转录本稳定性之间存在负相关的情况,但在这里我们发现较短的同工型不一定更稳定。我们证明了RNA-蛋白质相互作用在调节同工型特异性稳定性中的作用,表明PUF3结合并使特定的聚腺苷酸同工型不稳定。我们的发现表明,尽管基因的功能元件是在DNA序列中编码的,但通过转录本边界变化将这些元件选择性地掺入RNA允许单个基因产生多种功能后果。聚腺苷酸化。这项研究表明,每个基因的同工型可以具有不同的分子表型,如RNA稳定性和与蛋白质的相互作用,从而使基因组的功能潜力多样化.3'转录本同工型在转录后的命运在全基因组水平上有所揭示。本文提出了可以精确测量同工型特异性稳定性和蛋白质结合的方法,从而证明了两者的广泛差异。即使是几个核苷酸的变异也与转录本稳定性的变化有关。转录本与PUF3的结合以及随后的去稳定化是以同工型特异性的方式发生的。

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