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Hormone-induced and DNA Demethylation-induced Relief of a Tissue-specific and Developmentally Regulated Block in Transcriptional Elongation

机译:激素诱导和DNA去甲基化诱导的转录伸长中的组织特异性和发育调控块。

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摘要

Genome-wide studies have revealed that genes commonly have a high density of RNA polymerase II just downstream of the transcription start site. This has raised the possibility that genes are commonly regulated by transcriptional elongation, but this remains largely untested in vivo, particularly in vertebrates. Here, we show that the proximal promoter from the Rhox5 homeobox gene recruits polymerase II and begins elongating in all tissues and cell lines that we tested, but it only completes elongation in a tissue-specific and developmentally regulated manner. Relief of the elongation block is associated with recruitment of the elongation factor P-TEFb, the co-activator GRIP1, the chromatin remodeling factor BRG1, and specific histone modifications. We provide evidence that two mechanisms relieve the elongation block at the proximal promoter: demethylation and recruitment of androgen receptor. Together, our findings support a model in which promoter proximal pausing helps confer tissue-specific and developmental gene expression through a mechanism regulated by DNA demethylation-dependent nuclear hormone receptor recruitment.
机译:全基因组研究表明,基因通常在转录起始位点的下游具有高密度的RNA聚合酶II。这增加了基因通常受转录延伸调控的可能性,但这在体内尤其是在脊椎动物中仍然未经测试。在这里,我们显示了Rhox5同源框基因的近端启动子募集了聚合酶II,并在我们测试的所有组织和细胞系中开始延伸,但仅以组织特异性和发育调控的方式完成了延伸。延伸阻滞的缓解与延伸因子P-TEFb,共激活因子GRIP1,染色质重塑因子BRG1和特定组蛋白修饰的募集有关。我们提供的证据表明,两种机制可缓解近端启动子处的延伸阻滞:去甲基化和雄激素受体募集。在一起,我们的发现支持一个模型,其中启动子近端暂停通过DNA脱甲基依赖性核激素受体募集调节的机制,帮助赋予组织特异性和发育性基因表达。

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