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首页> 外文期刊>Nucleic Acids Research >Sub1 contacts the RNA polymerase II stalk to modulate mRNA synthesis
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Sub1 contacts the RNA polymerase II stalk to modulate mRNA synthesis

机译:Sub1接触RNA聚合酶II茎秆以调节mRNA合成

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摘要

Biogenesis of messenger RNA is critically influenced by the phosphorylation state of the carboxy-terminal domain (CTD) in the largest RNA polymerase II (RNAPII) subunit. Several kinases and phosphatases are required to maintain proper CTD phosphorylation levels and, additionally, several other proteins modulate them, including Rpb4/7 and Sub1. The Rpb4/7 heterodimer, constituting the RNAPII stalk, promote phosphatase functions and Sub1 globally influences CTD phosphorylation, though its mechanism remains mostly unknown. Here, we show that Sub1 physically interacts with the RNAPII stalk domain, Rpb4/7, likely through its C-terminal region, and associates with Fcp1. While Rpb4 is not required for Sub1 interaction with RNAPII complex, a fully functional heterodimer is required for Sub1 association to promoters. We also demonstrate that a complete CTD is necessary for proper association of Sub1 to chromatin and to the RNAPII. Finally, genetic data show a functional relationship between Sub1 and the RNAPII clamp domain. Altogether, our results indicate that Sub1, Rpb4/7 and Fcp1 interaction modulates CTD phosphorylation. In addition, Sub1 interaction with Rpb4/7 can also modulate transcription start site selection and transcription elongation rate likely by influencing the clamp function.
机译:信使RNA的生物发生受到最大RNA聚合酶II(RNAPII)亚基的羧基 - 末端结构域(CTD)的磷酸化状态的严重影响。需要几种激酶和磷酸酶来维持适当的CTD磷酸化水平,另外,其他几种蛋白质调节它们,包括RPB4 / 7和Sub1。 RPB4 / 7的异二聚体,构成RNAPII茎,促进磷酸酶功能和SUB1,影响CTD磷酸化,尽管其机制仍然是未知的。这里,我们表明Sub1与RNAPII轨迹域,可能通过其C终端区域的RPB4 / 7进行物理交互,以及与FCP1相关联。虽然Sub1与RNAPII复合物的子1相互作用不需要RPB4,但是对启动子的子1拟合需要全功能性异二聚体。我们还证明了完整的CTD是适当的SUB1至染色质和RNAPII的关联所必需的。最后,遗传数据显示了Sub1和RNAPII钳位结构域之间的功能关系。完全,我们的结果表明Sub1,RPB4 / 7和FCP1相互作用调节CTD磷酸化。另外,通过影响钳位功能,Sub1与RPB4 / 7的相互作用也可以调节转录开始点选择和转录伸长率。

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