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Two separate pathways regulate protein stability of ATM/ATR-related protein kinases Mec1 and Tel1 in budding yeast

机译:两条独立的途径调节芽苗中ATM / ATR相关蛋白激酶Mec1和Tel1的蛋白稳定性

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摘要

Checkpoint signaling requires two conserved phosphatidylinositol 3-kinase-related protein kinases (PIKKs): ATM and ATR. In budding yeast, Tel1 and Mec1 correspond to ATM and ATR, respectively. The Tel2-Tti1-Tti2 (TTT) complex connects to the Rvb1-Rvb2-Tah1-Pih1 (R2TP) complex for the protein stability of PIKKs; however, TTT-R2TP interaction only partially mediates ATM and ATR protein stabilization. How TTT controls protein stability of ATM and ATR remains to be precisely determined. Here we show that Asa1, like Tel2, plays a major role in stabilization of newly synthesized Mec1 and Tel1 proteins whereas Pih1 contributes to Mec1 and Tel1 stability at high temperatures. Although Asa1 and Pih1 both interact with Tel2, no Asa1-Pih1 interaction is detected. Pih1 is distributed in both the cytoplasm and nucleus wheres Asa1 localizes largely in the cytoplasm. Asa1 and Pih1 are required for proper DNA damage checkpoint signaling. Our findings provide a model in which two different Tel2 pathways promote protein stabilization of Mec1 and Tel1 in budding yeast.
机译:检查点信号传输需要两个保守的磷脂酰肌醇3激酶相关蛋白激酶(PIKK):ATM和ATR。在发芽酵母中,Tel1和Mec1分别对应于ATM和ATR。 Tel2-Tti1-Tti2(TTT)复合物与Rvb1-Rvb2-Tah1-Pih1(R2TP)复合物相连,以保证PIKK的蛋白质稳定性。但是,TTT-R2TP相互作用仅部分介导ATM和ATR蛋白质的稳定。 TTT如何控制ATM和ATR的蛋白质稳定性仍有待精确确定。在这里,我们显示Asa1像Tel2一样,在新合成的Mec1和Tel1蛋白质的稳定化中起主要作用,而Pih1有助于高温下Mec1和Tel1的稳定性。尽管Asa1和Pih1都与Tel2交互,但未检测到Asa1-Pih1交互。 Pih1分布在细胞质和细胞核中,而Asa1主要分布在细胞质中。正确的DNA损伤检查点信号转导需要Asa1和Pih1。我们的发现提供了一个模型,其中两个不同的Tel2途径促进了萌芽酵母中Mec1和Tel1的蛋白质稳定。

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