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DNA拓扑异构酶II是酵母着丝粒染色质拉伸特性和张力检查点的一个决定因素。

DNA topoisomerase II is a determinant of the tensile properties of yeast centromeric chromatin and the tension checkpoint.

作者信息

Warsi Tariq H, Navarro Michelle S, Bachant Jeff

机构信息

Department of Cell Biology and Neuroscience, University of California, Riverside, Riverside, CA 92521, USA.

出版信息

Mol Biol Cell. 2008 Oct;19(10):4421-33. doi: 10.1091/mbc.e08-05-0547. Epub 2008 Aug 13.

Abstract

Centromeric (CEN) chromatin is placed under mechanical tension and stretches as kinetochores biorient on the mitotic spindle. This deformation could conceivably provide a readout of biorientation to error correction mechanisms that monitor kinetochore-spindle interactions, but whether CEN chromatin acts in a tensiometer capacity is unresolved. Here, we report observations linking yeast Topoisomerase II (Top2) to both CEN mechanics and assessment of interkinetochore tension. First, in top2-4 and sumoylation-resistant top2-SNM mutants CEN chromatin stretches extensively during biorientation, resulting in increased sister kinetochore separation and preanaphase spindle extension. Our data indicate increased CEN stretching corresponds with alterations to CEN topology induced in response to tension. Second, Top2 potentiates aspects of the tension checkpoint. Mutations affecting the Mtw1 kinetochore protein activate Ipl1 kinase to detach kinetochores and induce spindle checkpoint arrest. In mtw1top2-4 and mtw1top2-SNM mutants, however, kinetochores are resistant to detachment and checkpoint arrest is attenuated. For top2-SNM cells, CEN stretching and checkpoint attenuation occur even in the absence of catenation linking sister chromatids. In sum, Top2 seems to play a novel role in CEN compaction that is distinct from decatenation. Perturbations to this function may allow weakened kinetochores to stretch CENs in a manner that mimics tension or evades Ipl1 surveillance.

摘要

着丝粒(CEN)染色质处于机械张力之下,并随着动粒在有丝分裂纺锤体上双定向排列而伸展。可以想象,这种变形可能为监测动粒-纺锤体相互作用的纠错机制提供双定向排列的读数,但CEN染色质是否以张力计的能力发挥作用仍未解决。在这里,我们报告了将酵母拓扑异构酶II(Top2)与CEN力学和动粒间张力评估联系起来的观察结果。首先,在top2-4和抗SUMO化的top2-SNM突变体中,CEN染色质在双定向排列过程中广泛伸展,导致姐妹动粒分离增加和前期纺锤体延伸。我们的数据表明,CEN伸展增加与因张力而诱导的CEN拓扑结构改变相对应。其次,Top2增强了张力检查点的某些方面。影响Mtw1动粒蛋白的突变激活Ipl1激酶以分离动粒并诱导纺锤体检查点停滞。然而,在mtw1top2-4和mtw1top2-SNM突变体中,动粒对分离具有抗性,检查点停滞减弱。对于top2-SNM细胞,即使在没有连接姐妹染色单体的连环结构的情况下,也会发生CEN伸展和检查点减弱。总之,Top2似乎在CEN压缩中发挥了一种与解连环作用不同的新作用。对该功能的干扰可能会使减弱的动粒以模仿张力或逃避Ipl1监测的方式拉伸CEN。

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