Myosin-1C associates with microtubules and stabilizes the mitotic spindle during cell division

Author:

Rump Agrani1,Scholz Tim2,Thiel Claudia1,Hartmann Falk K.1,Uta Petra2,Hinrichs Maike H.2,Taft Manuel H.1,Tsiavaliaris Georgios1

Affiliation:

1. Laboratory for Cellular Biophysics, Institute for Biophysical Chemistry, Hannover Medical School, 30625 Hannover, Germany

2. Institute for Molecular and Cell Physiology, Hannover Medical School, 30625 Hannover, Germany

Abstract

The mitotic spindle in eukaryotic cells is composed of a bipolar array of microtubules (MTs) and associated proteins that are required during mitosis for the correct partitioning of the two sets of chromosomes to the daughter cells. In addition to the well-established functions of MT-associated proteins (MAPs) and MT-based motors in cell division, there is increasing evidence that the F-actin-based myosin motors are important mediators of F-actin–MT interactions during mitosis. Here, we report the functional characterization of the long-tailed class-1 myosin myosin-1C from Dictyostelium discoideum during mitosis. Our data reveal that myosin-1C binds to MTs and has a role in maintenance of spindle stability for accurate chromosome separation. Both myosin-1C motor function and tail-domain-mediated MT–F-actin interactions are required for the cell-cycle-dependent relocalization of the protein from the cell periphery to the spindle. We show that the association of myosin-1C with MTs is mediated through the tail domain. The myosin-1C tail can inhibit kinesin motor activity, increase the stability of MTs, and form crosslinks between MTs and F-actin. These data illustrate that myosin-1C is involved in the regulation of MT function during mitosis in D. discoideum.

Publisher

The Company of Biologists

Subject

Cell Biology

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