Abstract

During cytokinesis, a contractile ring generates the constricting force to divide a cell into two daughters. This ring is composed of filamentous actin and the motor protein myosin, along with additional structural and regulatory proteins, including anillin. Anillin is a required scaffold protein that links the actomyosin ring to membrane and its organizer, RhoA. However, the molecular basis for timely action of anillin at cytokinesis remains obscure. Here, we find that phosphorylation regulates efficient recruitment of human anillin to the equatorial membrane. Anillin is highly phosphorylated in mitosis, and is a substrate for mitotic kinases. We surveyed function of 46 residues on anillin previously found to be phosphorylated in human cells to identify those required for cytokinesis. Among these sites, we identified S635 as a key site mediating cytokinesis. Preventing S635 phosphorylation adjacent to the AH domain disrupts anillin concentration at the equatorial cortex at anaphase, whereas a phosphomimetic mutant, S635D, partially restores this localization. Time-lapse videomicroscopy reveals impaired recruitment of S635A anillin to equatorial membrane and a transient unstable furrow followed by ultimate failure in cytokinesis. A phosphospecific antibody confirms phosphorylation at S635 in late cytokinesis, although it does not detect phosphorylation in early cytokinesis, possibly due to adjacent Y634 phosphorylation. Together, these findings reveal that anillin recruitment to the equatorial cortex at anaphase onset is enhanced by phosphorylation and promotes successful cytokinesis.

Highlights

  • In cytokinesis, cells assemble and stabilize an actomyosin ring between segregated chromosomes to generate daughter cells

  • Cells preserve their genetic integrity by strict coordination of cell membrane cleavage, with accurate separation of genetic material

  • Protein phosphorylation is a common mechanism regulating timing of events in mitosis; 46 phosphorylation sites have been mapped on anillin, their functional significance is PLOS Genetics | DOI:10.1371/journal.pgen

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Summary

Introduction

Cells assemble and stabilize an actomyosin ring between segregated chromosomes to generate daughter cells. Inactivation of cyclin-dependent kinase 1 (Cdk1) triggers recruitment of centralspindlin to the central spindle and adjacent equatorial cell membrane [3,4,5]. Centralspindlin recruits the RhoGEF, epithelial cell transforming sequence 2 (Ect2), to locally activate the small GTPase RhoA [2, 4, 6] which specifies localization of the contractile actomyosin ring [7]. Temporal recruitment and activation of the centralspindlin apparatus depends on phosphorylation, including Cdk1-dependent phosphorylation sites on mitotic kinesin-like protein 1 (MKLP1) and Ect, lost at anaphase onset [3, 6], and anaphase-specific recruitment of Plk through phosphorylation of protein regulating cytokinesis 1 (PRC1) [8].

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