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Controlling long-range genomic interactions at a native locus by targeted tethering of a looping factor

机译:通过循环因子的靶向束缚控制天然基因座的远程基因组相互作用

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Chromatin loops juxtapose distal enhancers with active promoters, but their molecular architecture and relationship with transcription remain unclear. In erythroid cells, the locus control region (LCR) and β-globin promoter form a chromatin loop that requires transcription factor GATA1 and the associated molecule Ldb1. We employed artificial zinc fingers (ZF) to tether Ldb1 to the β-globin promoter in GATA1 null erythroblasts, in which the β-globin locus is relaxed and inactive. Remarkably, targeting Ldb1 or only its self-association domain to the β-globin promoter substantially activated β-globin transcription in the absence of GATA1. Promoter-tethered Ldb1 interacted with endogenous Ldb1 complexes at the LCR to form a chromatin loop, causing recruitment and phosphorylation of RNA polymerase II. ZF-Ldb1 proteins were inactive at alleles lacking the LCR, demonstrating that their activities depend on long-range interactions. Our findings establish Ldb1 as a critical effector of GATA1-mediated loop formation and indicate that chromatin looping causally underlies gene regulation. PaperFlick
机译:染色质环将远端增强子与活性启动子并置,但它们的分子结构和与转录的关系仍不清楚。在类红细胞中,基因座控制区(LCR)和β-珠蛋白启动子形成一个染色质环,该环需要转录因子GATA1和相关分子Ldb1。我们使用人工锌指(ZF)将Ldb1拴系到GATA1空红细胞中的β-球蛋白启动子上,其中β-球蛋白的基因座是松弛的且无活性。值得注意的是,在不存在GATA1的情况下,将Ldb1或仅将其自缔合域靶向β-珠蛋白启动子可基本上激活β-珠蛋白的转录。启动子拴系的Ldb1在LCR处与内源性Ldb1复合物相互作用形成染色质环,从而引起RNA聚合酶II的募集和磷酸化。 ZF-Ldb1蛋白在缺少LCR的等位基因处无活性,表明它们的活性取决于远程相互作用。我们的发现将Ldb1确立为GATA1介导的环形成的关键效应子,并表明染色质环因果关系是基因调控的基础。 PaperFlick

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