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纺锤体检查点激活过程中,APC/C和Mad2介导的Cdc20降解。

APC/C- and Mad2-mediated degradation of Cdc20 during spindle checkpoint activation.

作者信息

Ge Sheng, Skaar Jeffrey R, Pagano Michele

机构信息

Department of Pathology, NYU Cancer Institute, New York University School of Medicine, 550 First Avenue, New York, NY 10016, USA.

出版信息

Cell Cycle. 2009 Jan 1;8(1):167-71. doi: 10.4161/cc.8.1.7606. Epub 2009 Jan 11.

DOI:10.4161/cc.8.1.7606
PMID:19098431
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2703714/
Abstract

The spindle assembly checkpoint (SAC) is an important mechanism that prevents the separation of sister chromatids until the microtubules radiating from the spindle poles are correctly attached to the kinetochores. Cdc20, an activator of the Anaphase Promoting Complex/Cyclosome (APC/C), is known as a major downstream target for inhibition by the SAC through the binding of mitotic checkpoint proteins, such as Mad2 and BubR1. Here, we report that the SAC negatively regulates the stability of Cdc20 by targeting it for proteasome-dependent degradation. Once the checkpoint is activated by spindle poisons, a major population of Cdc20 is degraded via APC/C, an event that requires the binding of Cdc20 to Mad2. We propose that the degradation of Cdc20 represents a critical control mechanism to ensure inactivation of APC/C(Cdc20) in response to the SAC.

摘要

纺锤体组装检验点(SAC)是一种重要机制,可防止姐妹染色单体分离,直到从纺锤体极发出的微管正确附着到动粒上。细胞分裂周期蛋白20(Cdc20)是后期促进复合物/细胞周期体(APC/C)的激活剂,通过有丝分裂检验点蛋白(如Mad2和BubR1)的结合,它是SAC抑制的主要下游靶点。在此,我们报告SAC通过靶向Cdc20进行蛋白酶体依赖性降解来负调控其稳定性。一旦检验点被纺锤体毒素激活,大量Cdc20会通过APC/C降解,这一事件需要Cdc20与Mad2结合。我们提出,Cdc20的降解代表了一种关键的控制机制,以确保响应SAC时APC/C(Cdc20)失活。

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