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XB-ART-51900
J Cell Sci 2016 Apr 01;1297:1329-39. doi: 10.1242/jcs.178855.
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Greatwall dephosphorylation and inactivation upon mitotic exit is triggered by PP1.

Ma S , Vigneron S , Robert P , Strub JM , Cianferani S , Castro A , Lorca T .


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Entry into mitosis is induced by the activation of cyclin-B-Cdk1 and Greatwall (Gwl; also known as MASTL in mammals) kinases. Cyclin-B-Cdk1 phosphorylates mitotic substrates, whereas Gwl activation promotes the phosphorylation of the small proteins Arpp19 and ENSA. Phosphorylated Arpp19 and/or ENSA bind to and inhibit PP2A comprising the B55 subunit (PP2A-B55; B55 is also known as PPP2R2A), the phosphatase responsible for cyclin-B-Cdk1 substrate dephosphorylation, allowing the stable phosphorylation of mitotic proteins. Upon mitotic exit, cyclin-B-Cdk1 and Gwl kinases are inactivated, and mitotic substrates are dephosphorylated. Here, we have identified protein phosphatase-1 (PP1) as the phosphatase involved in the dephosphorylation of the activating site (Ser875) of Gwl. Depletion of PP1 from meioticXenopusegg extracts maintains phosphorylation of Ser875, as well as the full activity of this kinase, resulting in a block of meiotic and mitotic exit. By contrast, preventing the reactivation of PP2A-B55 through the addition of a hyperactive Gwl mutant (GwlK72M) mainly affected Gwl dephosphorylation on Thr194, resulting in partial inactivation of Gwl and in the incomplete exit from mitosis or meiosis. We also show that when PP2A-B55 is fully reactivated by depleting Arpp19, this protein phosphatase is able to dephosphorylate both activating sites, even in the absence of PP1.

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Species referenced: Xenopus laevis
Genes referenced: arpp19 cdk1 ensa mastl mink1 npy4r ptpa
GO keywords: protein phosphatase 1 binding [+]
???displayArticle.antibodies??? Cdk1 Ab3 Mapk1 Ab20 Ppp1a Ab1 arpp19 Ab1 ctdp1 Ab1 ptpa Ab1 ptpa Ab2 ptpa Ab3


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