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Human centromere chromatin protein hMis12, essential for equal segregation, is independent of CENP-A loading pathway

机译:人类着丝粒染色质蛋白hMis12对平等隔离至关重要,独立于CENP-A加载途径

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Kinetochores are the chromosomal sites for spindle interaction and play a vital role for chromosome segregation. The composition of kinetochore proteins and their cellular roles are, however, poorly understood in higher eukaryotes. We identified a novel kinetochore protein family conserved from yeast to human that is essential for equal chromosome segregation. The human homologue hMis12 of yeast spMis12/scMtw1 retains conserved sequence features and locates at the kinetochore region indistinguishable from CENP-A, a centromeric histone variant. RNA interference (RNAi) analysis of HeLa cells shows that the reduced hMis12 results in misaligned metaphase chromosomes, lagging anaphase chromosomes, and interphase micronuclei without mitotic delay, while CENP-A is located at kinetochores. Further, the metaphase spindle length is abnormally extended. Spindle checkpoint protein hMad2 temporally localizes at kinetochores at early mitotic stages after RNAi. The RNAi deficiency of CENP-A leads to a similar mitotic phenotype, but the kinetochore signals of other kinetochore proteins, hMis6 and CENP-C, are greatly diminished. RNAi for hMis6, like that of a kinetochore kinesin CENP-E, induces mitotic arrest. Kinetochore localization of hMis12 is unaffected by CENP-A RNAi, demonstrating an independent pathway of CENP-A in human kinetochores.
机译:动植物是纺锤体相互作用的染色体位点,对染色体的分离起着至关重要的作用。然而,在高等真核生物中,对线粒体蛋白的组成及其在细胞中的作用知之甚少。我们确定了一个从酵母到人保守的新的线粒体蛋白家族,这对于相等的染色体分离至关重要。酵母spMis12 / scMtw1的人同源hMis12保留了保守的序列特征,并位于与着丝粒组蛋白变体CENP-A不可区分的动线粒区域。对HeLa细胞的RNA干扰(RNAi)分析表明,减少的hMis12导致错配的中期染色体,落后的后期染色体和无核分裂延迟的相间微核,而CENP-A位于动植物。此外,中期纺锤体长度异常延长。纺锤体检查点蛋白hMad2在RNAi后的有丝分裂早期在动粒体中暂时定位。 CENP-A的RNAi缺乏导致相似的有丝分裂表型,但是其他动线粒蛋白hMis6和CENP-C的动线粒信号大大减少。 hMis6的RNAi就像动粒动蛋白CENP-E一样,可诱导有丝分裂阻滞。 hMis12的线粒体定位不受CENP-A RNAi的影响,这表明CENP-A在人类动植物中的独立途径。

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