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High-density yeast-tiling array reveals previously undiscovered introns and extensive regulation of meiotic splicing

机译:高密度酵母平铺阵列显示以前未发现的内含子和减数分裂剪接的广泛调控

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摘要

Knowing gene structure is vital to understanding gene function, and accurate genome annotation is essential for understanding cellular function. To this end, we have developed a genome-wide assay for mapping introns in Saccharomyces cerevisiae. Using high-density tiling arrays, we compared wild-type yeast to a mutant deficient for intron degradation. Our method identified 76% of the known introns, confirmed 18 previously predicted introns, and revealed 9 formerly undiscovered introns. Furthermore, we discovered that all 13 meiosis-specific intronic yeast genes undergo regulated splicing, which provides posttranscrip-tional regulation of the genes involved in yeast cell differentiation. Moreover, we found that ≈16% of intronic genes in yeast are incompletely spliced during exponential growth in rich medium, which suggests that meiosis is not the only biological process regulated by splicing. Our tiling-array assay provides a snapshot of the spliced transcriptome in yeast. This robust methodology can be used to explore environmentally distinct splicing responses and should be readily adaptable to the study of other organisms, including humans.
机译:知道基因结构对于理解基因功能至关重要,而准确的基因组注释对于理解细胞功能至关重要。为此,我们已经开发了一种全基因组测定方法,用于定位酿酒酵母中的内含子。使用高密度切片阵列,我们将野生型酵母与缺乏内含子降解的突变体进行了比较。我们的方法鉴定了76%的已知内含子,确认了18个先前预测的内含子,并揭示了9个以前未发现的内含子。此外,我们发现所有13个减数分裂特异性内含子酵母基因都经过调控的剪接,这为参与酵母细胞分化的基因提供了转录后调控。此外,我们发现在丰富的培养基中指数生长期间,酵母中约16%的内含子基因未完全剪接,这表明减数分裂并非唯一受剪接调控的生物学过程。我们的平铺阵列检测提供了酵母中剪接的转录组的快照。这种强大的方法可用于探索环境不同的剪接反应,并且应易于适应其他生物(包括人类)的研究。

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