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Extensive Transcript Diversity and Novel Upstream Open Reading Frame Regulation in Yeast

机译:酵母中广泛的转录本多样性和新型上游开放阅读框调控

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摘要

To understand the diversity of transcripts in yeast (Saccharomyces cerevisiae) we analyzed the transcriptional landscapes for cells grown under 18 different environmental conditions. Each sample was analyzed using RNA-sequencing, and a total of 670,446,084 uniquely mapped reads and 377,263 poly-adenylated end tags were produced. Consistent with previous studies, we find that the majority of yeast genes are expressed under one or more different conditions. By directly comparing the 5′ and 3′ ends of the transcribed regions, we find extensive differences in transcript ends across many conditions, especially those of stationary phase, growth in grape juice, and salt stimulation, suggesting differential choice of transcription start and stop sites is pervasive in yeast. Relative to the exponential growth condition (i.e., YPAD), transcripts differing at the 5′ ends and 3′ ends are predicted to differ in their annotated start codon in 21 genes and their annotated stop codon in 63 genes. Many (431) upstream open reading frames (uORFs) are found in alternate 5′ ends and are significantly enriched in transcripts produced during the salt response. Mutational analysis of five genes with uORFs revealed that two sets of uORFs increase the expression of a reporter construct, indicating a role in activation which had not been reported previously, whereas two other uORFs decreased expression. In addition, RNA binding protein motifs are statistically enriched for alternate ends under many conditions. Overall, these results demonstrate enormous diversity of transcript ends, and that this heterogeneity is regulated under different environmental conditions. Moreover, transcript end diversity has important biological implications for the regulation of gene expression. In addition, our data also serve as a valuable resource for the scientific community.
机译:为了了解酵母(Saccharomyces cerevisiae)中转录本的多样性,我们分析了在18种不同环境条件下生长的细胞的转录情况。使用RNA测序对每个样品进行分析,共产生了670,446,084个唯一定位的读段和377,263个聚腺苷酸末端标签。与以前的研究一致,我们发现大多数酵母基因在一种或多种不同条件下表达。通过直接比较转录区的5'和3'末端,我们发现在许多条件下,尤其是在固定相,葡萄汁的生长和盐刺激下,转录末端的差异很大,这表明转录起始和终止位点的选择不同在酵母菌中很普遍。相对于指数生长条件(即,YPAD),在5'端和3'端不同的转录物预计在21个基因的注释起始密码子和在63个基因的注释终止密码子不同。在交替的5'末端发现了许多(431)上游开放阅读框(uORF),它们在盐反应期间产生的转录本中显着富集。对五个带有uORF的基因进行的突变分析表明,两组uORF均增加了报告基因构建体的表达,表明其在激活中的作用此前未见报道,而另外两个uORF则降低了表达。此外,在许多条件下,RNA结合蛋白基序在统计学上都丰富了可替代的末端。总的来说,这些结果证明了转录物末端的巨大多样性,并且这种异质性在不同的环境条件下受到调节。而且,转录物末端多样性对基因表达的调控具有重要的生物学意义。此外,我们的数据还为科学界提供了宝贵的资源。

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