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超分辨率动粒追踪揭示了人类姐妹动粒方向转换的机制。

Super-resolution kinetochore tracking reveals the mechanisms of human sister kinetochore directional switching.

作者信息

Burroughs Nigel J, Harry Edward F, McAinsh Andrew D

机构信息

Warwick Systems Biology Centre, Warwick Mathematics Institute, University of Warwick, Coventry, United Kingdom.

Warwick Molecular Organisation and Assembly in Cells, University of Warwick, Coventry, United Kingdom.

出版信息

Elife. 2015 Oct 13;4:e09500. doi: 10.7554/eLife.09500.

Abstract

The congression of chromosomes to the spindle equator involves the directed motility of bi-orientated sister kinetochores. Sister kinetochores bind bundles of dynamic microtubules and are physically connected through centromeric chromatin. A crucial question is to understand how sister kinetochores are coordinated to generate motility and directional switches. Here, we combine super-resolution tracking of kinetochores with automated switching-point detection to analyse sister switching dynamics over thousands of events. We discover that switching is initiated by both the leading (microtubules depolymerising) or trailing (microtubules polymerising) kinetochore. Surprisingly, trail-driven switching generates an overstretch of the chromatin that relaxes over the following half-period. This rules out the involvement of a tension sensor, the central premise of the long-standing tension-model. Instead, our data support a model in which clocks set the intrinsic-switching time of the two kinetochore-attached microtubule fibres, with the centromeric spring tension operating as a feedback to slow or accelerate the clocks.

摘要

染色体向纺锤体赤道面的汇聚涉及双定向姐妹动粒的定向运动。姐妹动粒结合动态微管束,并通过着丝粒染色质在物理上相连。一个关键问题是要了解姐妹动粒如何协同产生运动和方向转换。在这里,我们将动粒的超分辨率追踪与自动切换点检测相结合,以分析数千个事件中的姐妹切换动态。我们发现,切换由领先的(微管解聚)或落后的(微管聚合)动粒启动。令人惊讶的是,落后驱动的切换会使染色质过度拉伸,并在接下来的半个周期内松弛。这排除了张力传感器的参与,而张力传感器是长期存在的张力模型的核心前提。相反,我们的数据支持一种模型,即时钟设定两条动粒附着微管纤维的固有切换时间,着丝粒弹簧张力作为反馈来减慢或加速时钟。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3492/4764575/5537cd0effca/elife-09500-fig1.jpg

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