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p27Kip1 controls cytokinesis via the regulation of citron kinase activation
Murielle P. Serres, … , Nisar P. Malek, Arnaud Besson
Murielle P. Serres, … , Nisar P. Malek, Arnaud Besson
Published February 1, 2012
Citation Information: J Clin Invest. 2012;122(3):844-858. https://doi.org/10.1172/JCI60376.
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Research Article Oncology

p27Kip1 controls cytokinesis via the regulation of citron kinase activation

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Abstract

p27Kip1 (p27) acts as a tumor suppressor by inhibiting cyclin–cyclin-dependent kinase (cyclin-CDK) activity. However, mice expressing a form of p27 that is unable to bind or inhibit cyclin-CDK complexes (p27CK–) have increased incidence of tumor development as compared with wild-type and p27–/– mice, revealing an oncogenic role for p27. Here, we identified a phenotype of multinucleation and polyploidy in p27CK– mice not present in p27–/– animals, suggesting a role for p27 in G2/M that is independent of cyclin-CDK regulation. Further analysis revealed that p27CK– expression caused a cytokinesis and abscission defect in mouse embryonic fibroblasts. We identified the Rho effector citron kinase (citron-K) as a p27-interacting protein in vitro and in vivo and found that p27 and citron-K colocalized at the contractile ring and mid-body during telophase and cytokinesis. Moreover, overexpression of the minimal p27-binding domain of citron-K was sufficient to rescue the phenotype caused by p27CK–. Conversely, expression of a mutant p27CK– unable to bind citron-K did not induce multinucleation. Finally, by binding to citron-K, p27 prevented the interaction of citron-K with its activator RhoA. Taken together, these data suggest a role for p27 during cytokinesis via the regulation of citron-K activity.

Authors

Murielle P. Serres, Uta Kossatz, Yong Chi, James M. Roberts, Nisar P. Malek, Arnaud Besson

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Figure 5

Colocalization of p27 and citron-K at the mid-body.

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Colocalization of p27 and citron-K at the mid-body.
(A and B) After 24 h...
(A and B) After 24 hours in culture, HeLa cells were permeabilized with digitonin (40 μg/ml) before fixation. Mid-bodies were visualized with citron-K (goat anti–citron C20) staining in red (A) or green (B); p27 was detected with rabbit anti-p27 (C19) antibody in green (A) or red (B); and microtubules were stained with mouse anti–β-tubulin (purple) (original magnification, ×600). (C) HeLa cells were permeabilized with digitonin prior to fixation and stained with mouse anti-RhoA (26C4) antibody (green), rabbit anti-p27 (C19) (red), and goat anti-citron (C20) (purple) (original magnification, ×600). (D) Primary MEFs derived from p27+/+, p27–/–, and p27CK– mice were stained with anti-p27 (C19), anti-citron (C20), and anti–β-tubulin after digitonin permeabilization and fixation (original magnification, ×600).

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ISSN: 0021-9738 (print), 1558-8238 (online)

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