Literature DB >> 25661489

Sequential multisite phospho-regulation of KNL1-BUB3 interfaces at mitotic kinetochores.

Mathijs Vleugel1, Manja Omerzu2, Vincent Groenewold2, Michael A Hadders1, Susanne M A Lens1, Geert J P L Kops3.   

Abstract

Regulated recruitment of the kinase-adaptor complex BUB1/BUB3 to kinetochores is crucial for correcting faulty chromosome-spindle attachments and for spindle assembly checkpoint (SAC) signaling. BUB1/BUB3 localizes to kinetochores by binding phosphorylated MELT motifs (MELpT) in the kinetochore scaffold KNL1. Human KNL1 has 19 repeats that contain a MELT-like sequence. The repeats are, however, larger than MELT, and repeat sequences can vary significantly. Using systematic screening, we show that only a limited number of repeats is "active." Repeat activity correlates with the presence of a vertebrate-specific SHT motif C-terminal to the MELT sequence. SHT motifs are phosphorylated by MPS1 in a manner that requires prior phosphorylation of MELT. Phospho-SHT (SHpT) synergizes with MELpT in BUB3/BUB1 binding in vitro and in cells, and human BUB3 mutated in a predicted SHpT-binding surface cannot localize to kinetochores. Our data show sequential multisite regulation of the KNL1-BUB1/BUB3 interaction and provide mechanistic insight into evolution of the KNL1-BUB3 interface.
Copyright © 2015 Elsevier Inc. All rights reserved.

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Year:  2015        PMID: 25661489     DOI: 10.1016/j.molcel.2014.12.036

Source DB:  PubMed          Journal:  Mol Cell        ISSN: 1097-2765            Impact factor:   17.970


  52 in total

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Review 8.  Playing polo during mitosis: PLK1 takes the lead.

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Review 9.  The whole is greater than the sum of its parts: at the intersection of order, disorder, and kinetochore function.

Authors:  Margaux R Audett; Thomas J Maresca
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10.  Dynamic localization of Mps1 kinase to kinetochores is essential for accurate spindle microtubule attachment.

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