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PIAS1 regulates CP2c localization and active promoter complex formation in erythroid cell-specific α-globin expression

机译:PIAS1调节红细胞特异性α-珠蛋白表达中的CP2c定位和活性启动子复合物的形成

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摘要

Data presented here extends our previous observations on α-globin transcriptional regulation by the CP2 and PIAS1 proteins. Using RNAi knockdown, we have now shown that CP2b, CP2c and PIAS1 are each necessary for synergistic activation of endogenous α-globin gene expression in differentiating MEL cells. In this system, truncated PIAS1 mutants lacking the ring finger domain recruited CP2c to the nucleus, as did wild-type PIAS1, demonstrating that this is a sumoylation-independent process. In vitro, recombinant CP2c, CP2b and PIAS1 bound DNA as a stable CBP (CP2c/CP2b/PIAS1) complex. Following PIAS1 knockdown in MEL cells, however, the association of endogenous CP2c and CP2b with the α-globin promoter simultaneously decreased. By mapping the CP2b- and CP2c-binding domains on PIAS1, and the PIAS1-binding domains on CP2b and CP2c, we found that two regions of PIAS1 that interact with CP2c/CP2b are required for its co-activator function. We propose that CP2c, CP2b, and PIAS1 form a hexametric complex with two units each of CP2c, CP2b, and PIAS1, in which PIAS1 serves as a clamp between two CP2 proteins, while CP2c binds directly to the target DNA and CP2b mediates strong transactivation.
机译:本文提供的数据扩展了我们先前对CP2和PIAS1蛋白对α-珠蛋白转录调控的观察。使用RNAi敲低,我们现在已经证明CP2b,CP2c和PIAS1分别是分化的MEL细胞中内源性α-球蛋白基因表达协同激活所必需的。在该系统中,缺少无名指结构域的截短的PIAS1突变体(如野生型PIAS1一样)将CP2c募集到细胞核,表明这是一个与sumoylation无关的过程。在体外,重组CP2c,CP2b和PIAS1将DNA结合为稳定的CBP(CP2c / CP2b / PIAS1)复合物。然而,在MEL细胞中PIAS1敲低后,内源性CP2c和CP2b与α-珠蛋白启动子的关联同时下降。通过映射PIAS1上的CP2b和CP2c结合域以及CP2b和CP2c上的PIAS1结合域,我们发现PIAS1的两个与CP2c / CP2b相互作用的区域是其共激活子功能所必需的。我们建议CP2c,CP2b和PIAS1形成一个具有两个单元的六边形复合体,每个单元分别包含CP2c,CP2b和PIAS1,其中PIAS1充当两个CP2蛋白之间的钳位,而CP2c直接与目标DNA结合,CP2b介导强反式激活。

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