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一个张力非依赖的机制降低了着丝粒上 Aurora B 介导的磷酸化作用,该机制是由 CENP-E 在微管捕获时产生的。

A tension-independent mechanism reduces Aurora B-mediated phosphorylation upon microtubule capture by CENP-E at the kinetochore.

机构信息

a Department of Pathology and Cell Biology , Columbia University Vagelos College of Physicians and Surgeons , New York , NY , USA.

出版信息

Cell Cycle. 2019 Jun;18(12):1349-1363. doi: 10.1080/15384101.2019.1617615. Epub 2019 May 23.

Abstract

During mitosis, Aurora B kinase is required for forming proper bi-oriented kinetochore-microtubule attachments. Current models suggest that tension exerted between a pair of sister-kinetochores (inter-kinetochore stretch) produces a spatial separation of Aurora B kinase from kinetochore-associated microtubule binding substrates, such as the Knl1-Mis12-Ndc80 (KMN) network, resulting in a decrease of phosphorylation and, thus, an increase of affinity for microtubules. Using Single-Molecule High-Resolution Colocalization (SHREC) microscopy analysis of the kinetochore-associated motor CENP-E, we now show that CENP-E undergoes structural rearrangements prior to and after tension generation at the kinetochore, and displays a bi-modal Gaussian distribution on a pair of bi-oriented sister kinetochores. The conformational change of CENP-E depends on its microtubule-stimulated motor motility and the highly flexible coiled-coil between its motor and kinetochore-binding tail domains. Chemical inhibition of the motor motility or perturbations of the coiled-coil domain of CENP-E increases Aurora B-mediated Ndc80 phosphorylation in a tension-independent manner. Metaphase chromosome misalignment caused by CENP-E inhibition can be rescued by chemical inhibition of Aurora B kinase. Furthermore, a pair of monotelic sister-kinetochores shows asymmetric levels of Aurora B-mediated phosphorylation in mono-polar spindles depending on CENP-E motor activity. These results collectively suggest a tension-independent mechanism to reduce Aurora B-mediated phosphorylation of outer kinetochore components in response to microtubule capture by CENP-E.

摘要

在有丝分裂过程中,Aurora B 激酶对于形成适当的双定向动粒-微管附着是必需的。目前的模型表明,一对姐妹动粒(动粒间拉伸)之间产生的张力导致 Aurora B 激酶与动粒相关微管结合底物(如 Knl1-Mis12-Ndc80(KMN)网络)分离,从而导致磷酸化减少,因此与微管的亲和力增加。使用动粒相关马达 CENP-E 的单分子高分辨率共定位(SHREC)显微镜分析,我们现在表明,CENP-E 在动粒处产生张力之前和之后都会发生结构重排,并且在一对双定向姐妹动粒上显示出双峰高斯分布。CENP-E 的构象变化取决于其微管刺激的马达运动性以及其马达和动粒结合尾部结构域之间的高度灵活的卷曲螺旋。马达运动性的化学抑制或 CENP-E 的卷曲螺旋结构域的扰动以张力非依赖的方式增加 Aurora B 介导的 Ndc80 磷酸化。由 CENP-E 抑制引起的中期染色体错位可以通过化学抑制 Aurora B 激酶来挽救。此外,在单极纺锤体中,一对单极姐妹动粒根据 CENP-E 马达活性显示出不对称水平的 Aurora B 介导的磷酸化。这些结果共同表明,存在一种张力非依赖的机制,可减少 CENP-E 捕获微管时 Aurora B 介导的外动粒成分的磷酸化。

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