The chromosome passenger complex is required for fidelity of chromosome transmission and cytokinesis in meiosis of mouse oocytes
Abstract
The existence of two forms of the chromosome passenger complex (CPC) in the mammalian oocyte has meant that its role in female meiosis has remained unclear. Here we use loss- and gain-of function approaches to assess the meiotic functions of one of the shared components of these complexes, INCENP, and of the variable kinase subunits, Aurora B or Aurora C. We show that either the depletion of INCENP or the combined inhibition of Aurora kinases B and C activates the anaphase-promoting complex or cyclosome (APC/C) before chromosomes have properly congressed in meiosis I and also prevents cytokinesis and hence extrusion of the first polar body. Overexpression of Aurora C also advances APC/C activation and results in cytokinesis failure in a high proportion of oocytes, indicative of a dominant effect on CPC function. Together, this points to roles for the meiotic CPC in functions similar to the mitotic roles of the complex: correcting chromosome attachment to microtubules, facilitating the spindle-assembly checkpoint (SAC) function and enabling cytokinesis. Surprisingly, overexpression of Aurora B leads to a failure of APC/C activation, stabilization of securin and consequently a failure of chiasmate chromosomes to resolve – a dominant phenotype that is completely suppressed by depletion of INCENP. Taken together with the differential distribution of Aurora proteins B and C on chiasmate chromosomes, this points to differential functions of the two forms of CPC in regulating the separation of homologous chromosomes in meiosis I.
Additional Information
© 2010 The Company of Biologists. Accepted 2 September 2010. We thank Anna Ajduk for help in assaying Aurora B function in the second meiosis, Bernhard Strauss for help in establishing conditions for monitoring Securin degradation and Jonathan Pines for the gift of the Securin–GFP construct; we also thank Helen Bolton for examining the role of Aurora C in embryos and John Crang for help in compiling figures. This work was supported by a Wellcome Trust grant to M.Z.-G. and an MRC Programme Grant to D.M.G. B.S. held a Gates Foundation Studentship of the University of Cambridge. J.N. is supported by a MRC Career Development Fellowship. K.L.-H. was supported by the Alfred Benzon Stipend, Denmark (current address: Institute of Medical Biochemistry, Aarhus University, Denmark). Part of the image acquisition was carried out in the Wellcome-Trust-supported light microscopy facility in the University of Sheffield, UK (grant: GR077544AIA). Confocal microscope facilities in the D.M.G. laboratory were supported by grants from CR-UK and BBSRC. Deposited in PMC for release after 6 months. Supplementary material available online at http://jcs.biologists.org/lookup/suppl/doi:10.1242/jcs.067447/-/DC1Attached Files
Published - 4292.full.pdf
Supplemental Material - JCS067447FigS1.jpg
Supplemental Material - JCS067447FigS2.jpg
Supplemental Material - JCS067447FigS3.jpg
Supplemental Material - JCS067447FigS4.jpg
Supplemental Material - JCS067447FigS5.jpg
Supplemental Material - JCS067447TableS1.pdf
Supplemental Material - JCS067447TableS2.pdf
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Additional details
- PMCID
- PMC2995614
- Eprint ID
- 94768
- Resolver ID
- CaltechAUTHORS:20190417-163114460
- Wellcome Trust
- GR077544AIA
- Medical Research Council (UK)
- Bill and Melinda Gates Foundation
- Alfred Benzon Stipend, Denmark
- Cancer Research UK
- Biotechnology and Biological Sciences Research Council (BBSRC)
- Created
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2019-04-18Created from EPrint's datestamp field
- Updated
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2021-11-16Created from EPrint's last_modified field