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Cdc25 mitotic inducer targeted by chk1 DNA damage checkpoint kinase

机译:chk1 DNA损伤检查点激酶靶向的Cdc25有丝分裂诱导剂

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摘要

Arrest of the cell cycle at the G2 checkpoint, induced by DNA damage, requires inhibitory phosphorylation of the kinase Cdc2 in both fission yeast and human cells. The kinase Wee1 and the phosphatase Cdc25, which regulate Cdc2 phosphorylation, were evaluated as targets of Chk1, a kinase essential for the checkpoint. Fission yeast cdc2-3w Deltacdc25 cells, which express activated Cdc2 and lack Cdc25, were responsive to Wee1 but insensitive to Chk1 and irradiation. Expression of large amounts of Chk1 produced the same phenotype as did loss of the cdc25 gene in cdc2-3w cells. Cdc25 associated with Chk1 in vivo and was phosphorylated when copurified in Chk1 complexes. These findings identify Cdc25, but not Wee1, as a target of the DNA damage checkpoint.
机译:DNA损伤引起的G2检查点细胞周期的停止,要求裂变酵母和人类细胞中的Cdc2激酶具有抑制性磷酸化。调节Cdc2磷酸化的激酶Wee1和磷酸酶Cdc25被评估为Chk1(检查点必不可少的激酶)的靶标。裂变酵母cdc2-3w Deltacdc25细胞表达活化的Cdc2而缺乏Cdc25,它们对Wee1有反应,但对Chk1和辐射不敏感。大量Chk1的表达产生的表型与cdc2-3w细胞中cdc25基因的丢失相同。 Cdc25在体内与Chk1相关联,并在Chk1复合物中共纯化时被磷酸化。这些发现将Cdc25而非Wee1鉴定为DNA损伤检查点的靶标。

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