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Lack of Casein Kinase 1 Delta Promotes Genomic Instability - The Accumulation of DNA Damage and Down-Regulation of Checkpoint Kinase 1

机译:缺乏酪蛋白激酶1 Delta促进基因组不稳定 - DNa损伤的累积和检查点激酶1的下调

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摘要

Casein kinase 1 delta (CK1δ) is a conserved serine/threonine protein kinase that regulates diverse cellular processes. Mice lacking CK1δ have a perinatal lethal phenotype and typically weigh 30% less than their wild type littermates. However, the causes of death and small size are unknown. We observed cells with abnormally large nuclei in tissue from Csnk1d null embryos, and multiple centrosomes in mouse embryo fibroblasts (MEFs) deficient in CK1δ (MEFCsnk1d null). Results from γ-H2AX staining and the comet assay demonstrated significant DNA damage in MEFCsnk1d null cells. These cells often contain micronuclei, an indicator of genomic instability. Similarly, abrogation of CK1δ expression in control MEFs stimulated micronuclei formation after doxorubicin treatment, suggesting that CK1δ loss increases vulnerability to genotoxic stress. Cellular levels of total and activated checkpoint kinase 1 (Chk1), which functions in the DNA damage response and mitotic checkpoints, and its downstream effector, Cdc2/CDK1 kinase, were often decreased in MEFCsnk1d null cells as well as in control MEFs transfected with CK1δ siRNA. Hydroxyurea-induced Chk1 activation, as measured by Ser345 phosphorylation, and nuclear localization also were impaired in MEF cells following siRNA knockdown of CK1δ. Similar results were observed in the MCF7 human breast cancer cell line. The decreases in phosphorylated Chk1 were rescued by concomitant expression of siRNA-resistant CK1δ. Experiments with cycloheximide demonstrated that the stability of Chk1 protein was diminished in cells subjected to CK1δ knockdown. Together, these findings suggest that CK1δ contributes to the efficient repair of DNA damage and the proper functioning of mitotic checkpoints by maintaining appropriate levels of Chk1.
机译:酪蛋白激酶1δ(CK1δ)是一种保守的丝氨酸/苏氨酸蛋白激酶,可调节多种细胞过程。缺乏CK1δ的小鼠具有围产期致死表型,通常比野生型同窝小鼠轻30%。但是,死亡原因和体积小是未知的。我们观察到Csnk1d无效胚胎的组织中细胞核异常大,而CK1δ缺失的小鼠胚胎成纤维细胞(MEFs)的多个中心体(MEFCsnk1d无效)。 γ-H2AX染色和彗星试验的结果表明,MEFCsnk1d空细胞中存在明显的DNA损伤。这些细胞通常包含微核,这是基因组不稳定的指标。类似地,阿霉素处理后,对照MEF中CK1δ表达的消除刺激了微核的形成,这表明CK1δ的丧失增加了对遗传毒性胁迫的脆弱性。在DNA损伤反应和有丝分裂检查点中起作用的总和激活检查点激酶1(Chk1)的细胞水平及其下游效应子Cdc2 / CDK1激酶在MEFCsnk1d无效细胞以及经CK1δ转染的对照MEF中通常会降低siRNA。 siRNA敲低CK1δ后,MEF细胞中羟基脲诱导的Chk1活化(通过Ser345磷酸化测量)和核定位也受损。在MCF7人乳腺癌细胞系中观察到了相似的结果。磷酸化Chk1的减少通过siRNA抗性CK1δ的同时表达得以挽救。环己酰亚胺的实验表明,在经历CK1δ敲低的细胞中,Chk1蛋白的稳定性降低了。在一起,这些发现表明CK1δ通过维持适当的Chk1水平有助于DNA损伤的有效修复和有丝分裂检查点的正常运行。

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    Gao B;

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  • 年度 2017
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