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Control of meiotic pairing and recombination by chromosomally tethered 26S proteasome.


ABSTRACT: During meiosis, paired homologous chromosomes (homologs) become linked via the synaptonemal complex (SC) and crossovers. Crossovers mediate homolog segregation and arise from self-inflicted double-strand breaks (DSBs). Here, we identified a role for the proteasome, the multisubunit protease that degrades proteins in the nucleus and cytoplasm, in homolog juxtaposition and crossing over. Without proteasome function, homologs failed to pair and instead remained associated with nonhomologous chromosomes. Although dispensable for noncrossover formation, a functional proteasome was required for a coordinated transition that entails SC assembly between longitudinally organized chromosome axes and stable strand exchange of crossover-designated DSBs. Notably, proteolytic core and regulatory proteasome particles were recruited to chromosomes by Zip3, the ortholog of mammalian E3 ligase RNF212, and SC protein Zip1 . We conclude that proteasome functions along meiotic chromosomes are evolutionarily conserved.

SUBMITTER: Ahuja JS 

PROVIDER: S-EPMC6054871 | biostudies-literature | 2017 Jan

REPOSITORIES: biostudies-literature

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Control of meiotic pairing and recombination by chromosomally tethered 26S proteasome.

Ahuja Jasvinder S JS   Sandhu Rima R   Mainpal Rana R   Lawson Crystal C   Henley Hanna H   Hunt Patricia A PA   Yanowitz Judith L JL   Börner G Valentin GV  

Science (New York, N.Y.) 20170105 6323


During meiosis, paired homologous chromosomes (homologs) become linked via the synaptonemal complex (SC) and crossovers. Crossovers mediate homolog segregation and arise from self-inflicted double-strand breaks (DSBs). Here, we identified a role for the proteasome, the multisubunit protease that degrades proteins in the nucleus and cytoplasm, in homolog juxtaposition and crossing over. Without proteasome function, homologs failed to pair and instead remained associated with nonhomologous chromos  ...[more]

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