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着丝粒染色质的完整性因 Cdk5rap2 的缺失而受到损害,Cdk5rap2 是 CENP-A 的转录激活因子。

Centromeric chromatin integrity is compromised by loss of Cdk5rap2, a transcriptional activator of CENP-A.

机构信息

Department of Biochemistry & Molecular Biology, Harbin Medical University, Harbin, China; Department of Cell Biology & Anatomy, Arnie Charbonneau Cancer and Alberta Children's Hospital Research Institutes, Cumming School of Medicine, University of Calgary, Calgary, AB, Canada.

Department of Cell Biology & Anatomy, Arnie Charbonneau Cancer and Alberta Children's Hospital Research Institutes, Cumming School of Medicine, University of Calgary, Calgary, AB, Canada.

出版信息

Biomed Pharmacother. 2021 Jun;138:111463. doi: 10.1016/j.biopha.2021.111463. Epub 2021 Mar 13.

Abstract

Centromeres are chromosomal loci where kinetochores assemble to ensure faithful chromosome segregation during mitosis. CENP-A defines the loci by serving as an epigenetic marker that recruits other centromere components for a functional structure. However, the mechanism that controls CENP-A regulation of centromeric chromatin integrity remains to be explored. Separate studies have shown that loss of CENP-A or the Cdk5 regulatory subunit associated protein 2 (Cdk5rap2), a key player in mitotic progression, triggers the occurrence of lagging chromosomes. This prompted us to investigate a potential link between CENP-A and Cdk5rap2 in the maintenance of centromeric chromatin integrity. Here, we demonstrate that loss of Cdk5rap2 causes reduced CENP-A expression while exogenous Cdk5rap2 expression in cells depleted of endogenous Cdk5rap2 restores CENP-A expression. Indeed, we show that Cdk5rap2 is a nuclear protein that acts as a positive transcriptional regulator of CENP-A. Cdk5rap2 interacts with the CENP-A promoter and upregulates CENP-A transcription. Accordingly, loss of Cdk5rap2 causes reduced level of centromeric CENP-A. Exogenous CENP-A expression partially inhibits the occurrence of lagging chromosomes in Cdk5rap2 knockdown cells, indicating that lagging chromosomes induced by loss of Cdk5rap2 is due, in part, to loss of CENP-A. Aside from manifesting lagging chromosomes, cells depleted of Cdk5rap2, and thus CENP-A, show increased micronuclei and chromatin bridge formation. Altogether, our findings indicate that Cdk5rap2 serves to maintain centromeric chromatin integrity partly through CENP-A.

摘要

着丝粒是染色体上的位置,在有丝分裂过程中,动粒在这里组装以确保染色体的正确分离。CENP-A 通过作为表观遗传标记招募其他着丝粒成分来构建功能性结构,从而定义着丝粒位置。然而,控制 CENP-A 调节着丝粒染色质完整性的机制仍有待探索。单独的研究表明,CENP-A 或 Cdk5 调节亚基相关蛋白 2(Cdk5rap2)的缺失,Cdk5rap2 是有丝分裂进展的关键参与者,会触发滞后染色体的发生。这促使我们研究 CENP-A 和 Cdk5rap2 在维持着丝粒染色质完整性方面的潜在联系。在这里,我们证明 Cdk5rap2 的缺失导致 CENP-A 表达减少,而在耗尽内源性 Cdk5rap2 的细胞中外源表达 Cdk5rap2 则恢复 CENP-A 的表达。事实上,我们表明 Cdk5rap2 是一种核蛋白,它作为 CENP-A 的正转录调节因子发挥作用。Cdk5rap2 与 CENP-A 启动子相互作用并上调 CENP-A 转录。因此,Cdk5rap2 的缺失导致着丝粒 CENP-A 水平降低。外源性 CENP-A 表达部分抑制了 Cdk5rap2 敲低细胞中滞后染色体的发生,表明 Cdk5rap2 缺失引起的滞后染色体部分归因于 CENP-A 的缺失。除了表现出滞后染色体外,耗尽 Cdk5rap2 的细胞,从而耗尽 CENP-A,还显示出增加的微核和染色质桥形成。总之,我们的研究结果表明,Cdk5rap2 通过 CENP-A 部分维持着丝粒染色质完整性。

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