Microtubule end conversion mediated by motors and diffusing proteins with no intrinsic microtubule end-binding activity

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作者
Manas Chakraborty
Ekaterina V. Tarasovetc
Anatoly V. Zaytsev
Maxim Godzi
Ana C. Figueiredo
Fazly I. Ataullakhanov
Ekaterina L. Grishchuk
机构
[1] University of Pennsylvania,Department of Physiology, Perelman School of Medicine
[2] Russian Academy of Sciences,Center for Theoretical Problems of Physicochemical Pharmacology
[3] Universidade do Porto,Chromosome Instability & Dynamics Laboratory, Instituto de Biologia Molecular e Celular
[4] Universidade do Porto,Instituto de Investigação e Inovação em Saúde – i3S
[5] Dmitry Rogachev National Research Center of Pediatric Hematology,Centre for Mechanochemical Cell Biology
[6] Oncology and Immunology,undefined
[7] Moscow Institute of Physics and Technology,undefined
[8] Warwick Medical School,undefined
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摘要
Accurate chromosome segregation relies on microtubule end conversion, the ill-understood ability of kinetochores to transit from lateral microtubule attachment to durable association with dynamic microtubule plus-ends. The molecular requirements for this conversion and the underlying biophysical mechanisms are elusive. We reconstituted end conversion in vitro using two kinetochore components: the plus end–directed kinesin CENP-E and microtubule-binding Ndc80 complex, combined on the surface of a microbead. The primary role of CENP-E is to ensure close proximity between Ndc80 complexes and the microtubule plus-end, whereas Ndc80 complexes provide lasting microtubule association by diffusing on the microtubule wall near its tip. Together, these proteins mediate robust plus-end coupling during several rounds of microtubule dynamics, in the absence of any specialized tip-binding or regulatory proteins. Using a Brownian dynamics model, we show that end conversion is an emergent property of multimolecular ensembles of microtubule wall-binding proteins with finely tuned force-dependent motility characteristics.
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