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Basis of catalytic assembly of the mitotic checkpoint complex

机译:有丝分裂检查点复合物催化组装的基础

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摘要

In mitosis, for each daughter cell to inherit an accurate copy of the genome from the mother cell, sister chromatids in the mother cell must attach to microtubules emanating from opposite poles of the mitotic spindle, a process known as bi-orientation. A surveillance mechanism, termed the spindle assembly checkpoint (SAC), monitors the microtubule attachment process and can temporarily halt the separation of sister chromatids and the completion of mitosis until bi-orientation is complete(1). SAC failure results in abnormal chromosome numbers, termed aneuploidy, in the daughter cells, a hallmark of many tumours. The HORMA-domain-containing protein mitotic arrest deficient 2 (MAD2) is a subunit of the SAC effector mitotic checkpoint complex (MCC). Structural conversion from the open to the closed conformation of MAD2 is required for MAD2 to be incorporated into the MCC1. In vitro, MAD2 conversion and MCC assembly take several hours(2-4), but in cells the SAC response is established in a few minutes(5-7). Here, to address this discrepancy, we reconstituted a near-complete SAC signalling system with purified components and monitored assembly of the MCC in real time. A marked acceleration in MAD2 conversion and MCC assembly was observed when monopolar spindle 1 (MPS1) kinase phosphorylated the MAD1-MAD2 complex, triggering it to act as the template for MAD2 conversion and therefore contributing to the establishment of a physical platform for MCC assembly. Thus, catalytic activation of the SAC depends on regulated protein-protein interactions that accelerate the spontaneous but rate-limiting conversion of MAD2 required for MCC assembly.
机译:在有丝分裂中,为了使每个子细胞都能从母细胞继承基因组的精确副本,母细胞中的姊妹染色单体必须附着在有丝分裂纺锤体相反两极的微管上,这一过程称为双向取向。一种称为纺锤体装配检查点(SAC)的监视机制可以监视微管的附着过程,并可以暂时停止姐妹染色单体的分离和有丝分裂的完成,直至双向完成(1)。 SAC失败会在子细胞中导致异常染色体数目(称为非整倍性),这是许多肿瘤的标志。含HORMA域的蛋白质有丝分裂阻滞缺陷2(MAD2)是SAC效应子有丝分裂检查点复合物(MCC)的一个亚基。为了将MAD2整合到MCC1中,需要从MAD2的开放构象向封闭构象转换。在体外,MAD2转化和MCC组装需要几个小时(2-4),但是在细胞中,SAC反应会在几分钟内建立(5-7)。在这里,为了解决这一差异,我们重建了一个几乎完整的SAC信号系统,该系统具有纯化的组件并实时监控MCC的组装。当单极纺锤体1(MPS1)激酶磷酸化MAD1-MAD2复合物,触发其充当MAD2转化的模板时,观察到MAD2转化和MCC组装明显加速,从而有助于建立物理平台进行MCC组装。因此,SAC的催化活化取决于调节的蛋白质-蛋白质相互作用,该相互作用加速了MCC组装所需的MAD2的自发但速率受限的转化。

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  • 来源
    《Nature》 |2017年第7642期|498-502|共5页
  • 作者单位

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany;

    Max Planck Inst Mol Physiol, Dept Mech Cell Biol, Otto Hahn Str 11, D-44227 Dortmund, Germany|Univ Duisburg Essen, Ctr Med Biotechnol, Fac Biol, Univ Str, D-45141 Essen, Germany;

  • 收录信息 美国《科学引文索引》(SCI);美国《工程索引》(EI);美国《生物学医学文摘》(MEDLINE);美国《化学文摘》(CA);
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  • 正文语种 eng
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  • 入库时间 2022-08-18 02:51:43

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