| Literature DB >> 32130890 |
Wei He1, H B D Prasada Rao1, Shangming Tang1, Nikhil Bhagwat1, Dhananjaya S Kulkarni1, Yunmei Ma1, Maria A W Chang2, Christie Hall2, Junxi Wang Bragg2, Harrison S Manasca2, Christa Baker2, Gerrik F Verhees2, Lepakshi Ranjha3, Xiangyu Chen4, Nancy M Hollingsworth4, Petr Cejka3, Neil Hunter5.
Abstract
Crossover recombination is essential for accurate chromosome segregation during meiosis. The MutSγ complex, Msh4-Msh5, facilitates crossing over by binding and stabilizing nascent recombination intermediates. We show that these activities are governed by regulated proteolysis. MutSγ is initially inactive for crossing over due to an N-terminal degron on Msh4 that renders it unstable by directly targeting proteasomal degradation. Activation of MutSγ requires the Dbf4-dependent kinase Cdc7 (DDK), which directly phosphorylates and thereby neutralizes the Msh4 degron. Genetic requirements for Msh4 phosphorylation indicate that DDK targets MutSγ only after it has bound to nascent joint molecules (JMs) in the context of synapsing chromosomes. Overexpression studies confirm that the steady-state level of Msh4, not phosphorylation per se, is the critical determinant for crossing over. At the DNA level, Msh4 phosphorylation enables the formation and crossover-biased resolution of double-Holliday Junction intermediates. Our study establishes regulated protein degradation as a fundamental mechanism underlying meiotic crossing over.Entities:
Keywords: Cdc7; Holliday Junction; MutS; aneuploidy; chromosome; crossing over; degron; homologous recombination; meiosis; proteasome
Year: 2020 PMID: 32130890 PMCID: PMC7289160 DOI: 10.1016/j.molcel.2020.02.001
Source DB: PubMed Journal: Mol Cell ISSN: 1097-2765 Impact factor: 17.970