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Regulation of Chk1 Kinase by Autoinhibition and ATR-mediated Phosphorylation

机译:通过自动抑制和ATR介导的磷酸化调节Chk1激酶。

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The checkpoint kinase Chk1 undergoes ATR-mediated phosphorylation and activation in response to unreplicated DNA, but the precise mechanism of Chk1 activation is not known. In this study, we have analyzed the domain structure of Xenopus Chk1 and explored the mechanism of its activation by ATR-mediated phosphorylation. We show that the C-terminal region of Xenopus Chk1 contains an autoinhibitory region (AIR), which largely overlaps with a bipartite, unusually long (~85-amino acid) nuclear localization signal. When coexpressed in oocytes or embryos, the AIR can interact with and inhibit the kinase domain of Chk1, but not full-length Chk1, suggesting an autoinhibitory intramolecular interaction in the Chk1 molecule. If linked with the preceding ATR phosphorylation domain that has either phospho-mimic mutation or genuine phosphorylation, however, the AIR can no longer interact with or inhibit the kinase domain, suggesting a conformational change of the AIR by ATR-mediated phosphorylation. Even in full-length Chk1, such phospho-mimic mutation can interfere with the autoinhibitory intramolecular interaction, but only if this interaction is somewhat weakened by an additional mutation in the AIR. These results provide significant insights into the mechanism of Chk1 activation at the DNA replication checkpoint.
机译:检查点激酶Chk1响应未复制的DNA经历ATR介导的磷酸化和激活,但是Chk1激活的确切机制尚不清楚。在这项研究中,我们分析了非洲爪蟾Chk1的域结构,并探讨了其通过ATR介导的磷酸化激活的机制。我们显示,非洲爪蟾Chk1的C端区域包含一个自动抑制区域(AIR),该区域与二分体,异常长的(〜85个氨基酸)核定位信号很大程度上重叠。当在卵母细胞或胚胎中共表达时,AIR可以与Chk1的激酶结构域相互作用,但不能与全长的Chk1的激酶结构域相互作用,从而抑制Chk1分子中的自抑制分子内相互作用。但是,如果与具有磷酸化模拟突变或真正的磷酸化作用的先前的ATR磷酸化结构域连接,则AIR不再能够与激酶结构域相互作用或抑制激酶结构域,表明AIR通过ATR介导的磷酸化发生构象变化。即使在全长的Chk1中,这种磷酸化模拟突变也可以干扰自身抑制性分子内相互作用,但前提是这种相互作用会由于AIR中的其他突变而有所减弱。这些结果为在DNA复制检查点激活Chk1的机制提供了重要的见识。

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