首页> 外文期刊>Journal of Biophysical and Biochemical Cytology >53BP1 and USP28 mediate p53 activation and G1 arrest after centrosome loss or extended mitotic duration
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53BP1 and USP28 mediate p53 activation and G1 arrest after centrosome loss or extended mitotic duration

机译:53bp1和USP28介导P53激活和Centosome损失或延长有丝分裂持续时间后的G1停止

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In normal human cells, centrosome loss induced by centrinone—a specific centrosome duplication inhibitor—leads to irreversible, p53-dependent G1 arrest by an unknown mechanism. A genome-wide CRISPR/Cas9 screen for centrinone resistance identified genes encoding the p53-binding protein 53BP1, the deubiquitinase USP28, and the ubiquitin ligase TRIM37. Deletion of TP53BP1 , USP28 , or TRIM37 prevented p53 elevation in response to centrosome loss but did not affect cytokinesis failure–induced arrest or p53 elevation after doxorubicin-induced DNA damage. Deletion of TP53BP1 and USP28 , but not TRIM37 , prevented growth arrest in response to prolonged mitotic duration. TRIM37 knockout cells formed ectopic centrosomal-component foci that suppressed mitotic defects associated with centrosome loss. TP53BP1 and USP28 knockouts exhibited compromised proliferation after centrosome removal, suggesting that centrosome-independent proliferation is not conferred solely by the inability to sense centrosome loss. Thus, analysis of centrinone resistance identified a 53BP1-USP28 module as critical for communicating mitotic challenges to the p53 circuit and TRIM37 as an enforcer of the singularity of centrosome assembly.
机译:在正常的人体细胞中,Centrinone-A特异性中心组重复抑制剂引起的中心损失导致不可逆,P53依赖性G1通过未知机制被捕。用于中心抗蛋白质的基因组CRISPR / CAS9筛网,其鉴定了编码p53结合蛋白53bp1,氘素酶USP28和泛素连接酶TRIM37的基因。删除TP53BP1,USP28或TRIM37防止了P53升高以响应中心损失,但在多柔比蛋白诱导的DNA损伤后,不影响细胞因子衰竭诱导的逮捕或P53升高。缺失TP53BP1和USP28,但不是TRIM37,防止了增长逮捕,以响应长期的有丝分裂持续时间。 Trim37敲除细胞形成异位型中心组分灶,抑制与中心损失相关的有偶联缺陷。 TP53BP1和USP28敲除在拆除中心拆除后表现出受损的增殖,表明不完全赋予离心体的增殖,无法感知中心损失。因此,对中心电阻的分析鉴定了53bp1-USP28模块,以便为P53电路和Trim37传达有丝分裂挑战,作为中心组装的奇异性的强制性。

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