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CK2-mediated stimulation of Pol I transcription by stabilization of UBFSL1 interaction

机译:CK2介导的UBFSL1相互作用稳定刺激Pol I转录

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摘要

High levels of rRNA synthesis by RNA polymerase I are important for cell growth and proliferation. In vitro studies have indicated that the formation of a stable complex between the HMG box factor [Upstream binding factor (UBF)] and SL1 at the rRNA gene promoter is necessary to direct multiple rounds of Pol I transcription initiation. The recruitment of SL1 to the promoter occurs through protein interactions with UBF and is regulated by phosphorylation of UBF. Here we show that the protein kinase CK2co-immunoprecipitates with the Pol I complex and is associated with the rRNA gene promoter. Inhibition of CK2 kinase activity reduces Pol I transcription in cultured cells and in vitro. Significantly, CK2 regulates the interaction between UBF and SL1 bycounteracting the inhibitory effect of HMG boxes five and six through the phosphorylation of specific serines located at the C-terminus of UBF. Transcription reactions with immobilized templates indicate that phosphorylation of CK2 phosphoacceptor sitesin the C-terminal domain of UBF is important for promoting multiple rounds of Pol I transcription. These data demonstrate that CK2 is recruited to the rRNA gene promoter and directly regulates Pol I transcription re-initiation by stabilizing the association between UBF and SL1.
机译:RNA聚合酶I高水平合成rRNA对于细胞生长和增殖很重要。体外研究表明,rMG基因启动子在HMG盒因子[上游结合因子(UBF)]和SL1之间形成稳定的复合物对于指导多轮Pol I转录起始是必要的。 SL1向启动子的募集通过与UBF的蛋白质相互作用而发生,并受UBF磷酸化的调控。在这里,我们显示蛋白激酶CK2co-免疫沉淀与Pol I复合物并与rRNA基因启动子相关。 CK2激酶活性的抑制降低了培养细胞和体外的Pol I转录。重要的是,CK2通过抵消位于UBF C端的特定丝氨酸的磷酸化来抵消HMG盒5和6的抑制作用,从而调节UBF和SL1之间的相互作用。具有固定模板的转录反应表明,UBF C末端域中CK2磷酸受体位点的磷酸化对于促进多轮Pol I转录很重要。这些数据表明CK2被募集到rRNA基因启动子,并通过稳定UBF和SL1之间的缔合直接调节Pol I转录的重新启动。

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