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Uncoupling of the spindle-checkpoint and chromosome-congression functions of BubR1

机译:解旋主轴检查点和BubR1的染色体 - 会聚功能

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摘要

The BubR1 checkpoint protein performs multiple functions in mitosis. We have carried out a functional analysis of conserved motifs of human BubR1 (also known as BUB1B) and demonstrate that spindle assembly checkpoint (SAC) and chromosome attachment functions can be uncoupled from each other. Mutation of five proline-directed serine phosphorylation sites, identified in vivo by mass spectrometry, essentially abolishes attachment of chromosomes to the spindle but has no effect on SAC functionality. By contrast, mutation of the two conserved KEN boxes required for SAC function does not impact chromosome congression. Interestingly, the contribution of the two KEN-box motifs is not equal. Cdc20 associates with the N-terminal but not C-terminal KEN box, and mutation of the N-terminal KEN motif results in more severe acceleration of mitotic timing. Moreover, the two KEN motifs are not sufficient for maximal binding of Cdc20 and APC/C, which also requires sequences in the BubR1 C-terminus. Finally, mutation of the GLEBS motif causes loss of Bub3 interaction and mislocalization of BubR1 from the kinetochore; concomitantly, BubR1 phosphorylation as well as SAC activity and chromosome congression are impaired, indicating that the GLEBS motif is strictly required for both major functions of human BubR1.
机译:BubR1检查点蛋白在有丝分裂中具有多种功能。我们已经对人类BubR1(也称为BUB1B)的保守基序进行了功能分析,并证明了纺锤体装配检查点(SAC)和染色体附着功能可以彼此分离。通过质谱在体内鉴定出的五个脯氨酸定向的丝氨酸磷酸化位点的突变基本上消除了染色体与纺锤体的附着,但对SAC功能没有影响。相比之下,SAC功能所需的两个保守KEN盒的突变不会影响染色体国会。有趣的是,两个KEN-box图案的贡献不相等。 Cdc20与N末端而不是C末端KEN框相关联,并且N末端KEN基序的突变导致有丝分裂时机更严重的加速。此外,两个KEN基序不足以最大程度地结合Cdc20和APC / C,这也需要BubR1 C末端的序列。最后,GLEBS基序的突变会导致Bub3相互作用的丧失和BubR1在动粒上的定位错误;随之而来的是,BubR1的磷酸化以及SAC活性和染色体转换受到损害,表明GLEBS基序是人类BubR1的两个主要功能所必需的。

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