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Published January 2, 2018 | Supplemental Material + Published
Journal Article Open

Cyclin B1 is essential for mitosis in mouse embryos, and its nuclear export sets the time for mitosis

Abstract

There is remarkable redundancy between the Cyclin–Cdk complexes that comprise the cell cycle machinery. None of the mammalian A-, D-, or E-type cyclins are required in development until implantation, and only Cdk1 is essential for early cell divisions. Cyclin B1 is essential for development, but whether it is required for cell division is contentious. Here, we used a novel imaging approach to analyze Cyclin B1–null embryos from fertilization onward. We show that Cyclin B1−/− embryos arrest in G2 phase after just two divisions. This is the earliest arrest of any Cyclin known and places Cyclin B1 with cdk1 as the essential regulators of the cell cycle. We reintroduced mutant proteins into this genetically null background to determine why Cyclin B1 is constantly exported from the nucleus. We found that Cyclin B1 must be exported from the nucleus for the cell to prevent premature entry to mitosis, and retaining Cyclin B1–Cdk1 at the plasma membrane precludes entry to mitosis.

Additional Information

© 2018 Strauss et al. This article is available under a Creative Commons License (Attribution 4.0 International, as described at https://creativecommons.org/licenses/by/4.0/). Submitted: 20 December 2016. Revised: 2 August 2017. Accepted: 21 September 2017. We are very grateful to Jane Kirk and Tim Hunt for the gift of the Cyclin B1^(+/−) and Cyclin B2^(−/−) mouse strains. We thank all members of both our laboratories for help and advice. This work was supported by a Wellcome Trust Senior Fellowship to M. Zernicka-Goetz and subsequently by a program grant from the Medical Research Council to J. Pines. Both M. Zernicka-Goetz and J. Pines acknowledge core funding provided by the Wellcome Trust (092096) and Cancer Research UK (C6946/A14492). The authors declare no competing financial interests.

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Supplemental Material - JCB_201612147_sm.pdf

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Additional details

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