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Widespread transcriptional pausing and elongation control at enhancers

机译:增强剂的广泛转录暂停和伸长控制

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Regulation by gene-distal enhancers is critical for cell type-specific and condition-specific patterns of gene expression. Thus, to understand the basis of gene activity in a given cell type or tissue, we must identify the precise locations of enhancers and functionally characterize their behaviors. Here, we demonstrate that transcription is a nearly universal feature of enhancers in Drosophila and mammalian cells and that nascent RNA sequencing strategies are optimal for identification of both enhancers and superenhancers. We dissect the mechanisms governing enhancer transcription and discover remarkable similarities to transcription at protein-coding genes. We show that RNA polymerase II (RNAPII) undergoes regulated pausing and release at enhancers. However, as compared with mRNA genes, RNAPII at enhancers is less stable and more prone to early termination. Furthermore, we found that the level of histone H3 Lys4 (H3K4) methylation at enhancers corresponds to transcriptional activity such that highly active enhancers display H3K4 trimethylation rather than the H3K4 monomethylation considered a hallmark of enhancers. Finally, our work provides insights into the unique characteristics of superenhancers, which stimulate high-level gene expression through rapid pause release; interestingly, this property renders associated genes resistant to the loss of factors that stabilize paused RNAPII.
机译:基因远端增强剂的调节对于基因表达的细胞类型特异性和疾病特异性模式至关重要。因此,要了解给定细胞类型或组织中基因活性的基础,我们必须识别增强剂的精确位置,并在功能性地表征其行为。在这里,我们证明转录是果蝇和哺乳动物细胞中增强剂的几乎普遍的特征,并且新生的RNA测序策略是鉴定增强剂和超强州的最佳选择。解剖治疗增强剂转录的机制,并发现蛋白质编码基因的转录出现卓越的相似性。我们表明RNA聚合酶II(RNAPII)在增强剂中进行调节暂停和释放。然而,与mRNA基因相比,增强剂的RNAPII不太稳定,易于早期终止。此外,我们发现增强剂的组蛋白H3 Lys4(H3K4)甲基化水平对应于转录活性,使得高活性增强剂显示H3K4三甲基化而不是H3K4单甲基化被认为是增强剂的标志。最后,我们的工作提供了洞察过度的超强州的独特特征,通过快速暂停释放刺激高级基因表达;有趣的是,这种财产使相关基因抵抗稳定暂停RNAPII的因素的丧失。

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