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激光显微手术为缺乏 Pcs1 或 Clr4 的裂变酵母细胞中的 merotelic 动粒附着提供了证据。

Laser microsurgery provides evidence for merotelic kinetochore attachments in fission yeast cells lacking Pcs1 or Clr4.

机构信息

Max F. Perutz Laboratories, University of Vienna, Vienna, Austria.

出版信息

Cell Cycle. 2010 Oct 1;9(19):3997-4004. doi: 10.4161/cc.9.19.13233. Epub 2010 Oct 3.

Abstract

In order to segregate chromosomes properly, the cell must prevent merotelic kinetochore attachment, an error that occurs when a single kinetochore is attached to microtubules emanating from both spindle poles. Merotelic kinetochore orientation represents a major mechanism of aneuploidy in mitotic mammalian cells and it is the primary mechanism of chromosome instability in cancer cells. Fission yeast mutants defective in putative microtubule-site clamp Pcs1/Mde4 or Clr4/Swi6-dependent centromeric heterochromatin display high frequencies of lagging chromosomes during anaphase. Here, we developed an assay based on laser microsurgery to show that the stretched morphology of lagging kinetochores in pcs1Δ and clr4Δ mutant cells is due to merotelic attachment. We further show that Mde4 is regulated by Cdc2 and that Cdc2 activity prevents precocious localization of Mde4 to the metaphase spindle. Finally, we show that Pcs1/Mde4 complex shares similar features with the conserved kinetochore complex Spc24/Spc25 suggesting that these two complexes may occupy a similar functional niche.

摘要

为了正确分离染色体,细胞必须防止微管附着错误,即当一个动粒附着在来自纺锤体两极的微管上时发生的错误。微管附着错误是有丝分裂哺乳动物细胞非整倍体的主要机制,也是癌细胞染色体不稳定的主要机制。在裂殖酵母突变体中,假定的微管位点夹子 Pcs1/Mde4 或 Clr4/Swi6 依赖的着丝粒异染色质缺陷显示在后期有很高的滞后染色体频率。在这里,我们开发了一种基于激光显微手术的测定法,表明 pcs1Δ 和 clr4Δ 突变细胞中滞后动粒的拉伸形态是由于微管附着错误。我们进一步表明,Mde4 受 Cdc2 调控,Cdc2 活性阻止 Mde4 过早定位到中期纺锤体。最后,我们表明 Pcs1/Mde4 复合物与保守的动粒复合物 Spc24/Spc25 具有相似的特征,表明这两个复合物可能占据类似的功能位置。

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