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Alternative CDC20 translational isoforms tune mitotic arrest duration

Author

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  • Mary-Jane Tsang

    (Whitehead Institute for Biomedical Research
    Massachusetts Institute of Technology)

  • Iain M. Cheeseman

    (Whitehead Institute for Biomedical Research
    Massachusetts Institute of Technology)

Abstract

Mitotic defects activate the spindle-assembly checkpoint, which inhibits the anaphase-promoting complex co-activator CDC20 to induce a prolonged cell cycle arrest1,2. Once errors are corrected, the spindle-assembly checkpoint is silenced, allowing anaphase onset to occur. However, in the presence of persistent unresolvable errors, cells can undergo ‘mitotic slippage’, exiting mitosis into a tetraploid G1 state and escaping the cell death that results from a prolonged arrest. The molecular logic that enables cells to balance these duelling mitotic arrest and slippage behaviours remains unclear. Here we demonstrate that human cells modulate the duration of their mitotic arrest through the presence of conserved, alternative CDC20 translational isoforms. Downstream translation initiation results in a truncated CDC20 isoform that is resistant to spindle-assembly-checkpoint-mediated inhibition and promotes mitotic exit even in the presence of mitotic perturbations. Our study supports a model in which the relative levels of CDC20 translational isoforms control the duration of mitotic arrest. During a prolonged mitotic arrest, new protein synthesis and differential CDC20 isoform turnover create a timer, with mitotic exit occurring once the truncated Met43 isoform achieves sufficient levels. Targeted molecular changes or naturally occurring cancer mutations that alter CDC20 isoform ratios or its translational control modulate mitotic arrest duration and anti-mitotic drug sensitivity, with potential implications for the diagnosis and treatment of human cancers.

Suggested Citation

  • Mary-Jane Tsang & Iain M. Cheeseman, 2023. "Alternative CDC20 translational isoforms tune mitotic arrest duration," Nature, Nature, vol. 617(7959), pages 154-161, May.
  • Handle: RePEc:nat:nature:v:617:y:2023:i:7959:d:10.1038_s41586-023-05943-7
    DOI: 10.1038/s41586-023-05943-7
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