4.8 Article

Terminal cytokinesis events uncovered after an RNAi screen

Journal

CURRENT BIOLOGY
Volume 14, Issue 18, Pages 1685-1693

Publisher

CELL PRESS
DOI: 10.1016/j.cub.2004.08.063

Keywords

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Funding

  1. NIAID NIH HHS [R01 AI060102-05, R01 AI060102] Funding Source: Medline
  2. NIGMS NIH HHS [R01 GM037193-17, R01 GM037193-19, R37 GM037193, R01 GM060988, R01 GM037193, GM60988, GM371963, R01 GM037193-18, R01 GM060988-04] Funding Source: Medline

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Much of our understanding of animal cell cytokinesis centers on the regulation of the equatorial acto-myosin contractile ring that drives the rapid ingression of a deep cleavage furrow [1-5]. However, the central part of the mitotic spindle collapses to a dense structure that impedes the furrow and keeps the daughter cells connected via an intercellular bridge. Factors involved in the formation, maintenance, and resolution of this bridge are largely unknown [6]. Using a library of 7,216 double-stranded RNAs (dsRNAs) representing the conserved genes of Drosophila, we performed an RNA interference (RNAQ screen for cytokinesis genes in Schneider's S2 cells. We identified both familiar and novel genes whose inactivation induced a multi-nucleate phenotype. Using live video microscopy, we show that three genes: anillin, citron-kinase (CG10522), and soluble N-ethylmaleimide sensitive factor (NSF) attachmentprotein (alpha-SNAP), are essential forthe terminal (post-furrowing) events of cytokinesis. anillin RNAi caused gradual disruption of the intercellular bridge after furrowing; citron-kinase RNAi destabilized the bridge at a later stage; alpha-SNAP RNAi caused sister cells to fuse many hours later and by a different mechanism. We have shown that the stability of the intercellular bridge is essential for successful cytokinesis and have defined genes contributing to this stability.

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