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Roles of mammalian sterile 20‐like kinase 2‐dependent phosphorylations of Mps one binder 1B in the activation of nuclear Dbf2‐related kinases
Authors:Yijun Bao  Kazutaka Sumita  Takumi Kudo  Kanchanamala Withanage  Kentaro Nakagawa  Mitsunobu Ikeda  Kikuo Ohno  Yunjie Wang  Yutaka Hata
Affiliation:1. Department of Medical Biochemistry, Tokyo Medical and Dental University, Tokyo 113‐8519, Japan;2. Department of Neurosurgery, First Hospital of China Medical University, Shenyang 110001, China;3. Communicated by: Kohei Miyazono;4. Department of Neurosurgery, Graduate School of Medicine, Tokyo Medical and Dental University, Tokyo 113‐8519, Japan;5. Center for Brain Integration Research, Tokyo Medical and Dental University, Tokyo 113‐8519, Japan
Abstract:
Mammalian nuclear Dbf2‐related (NDR) kinases (LATS1, LATS2, NDR1 and NDR2) play a role in cell proliferation, apoptosis and morphological changes. Mammalian sterile 20‐like (MST) kinases and Mps one binder (MOB) proteins are important in the activation of NDR kinases. MOB1 is phosphorylated by MST1 and MST2 and this phosphorylation enhances the ability of MOB1 to activate NDR kinases. The phosphorylated MOB1 can be more effective as a scaffold protein to facilitate the MST‐dependent phosphorylation of NDR kinases and/or as a direct activator of NDR kinases. We previously reported that Thr74 of MOB1B is phosphorylated by MST2. Thr12 and Thr35 have also been identified as phosphorylation sites. In this study, we quantified the phosphorylation of Thr74 using the phosphorylated Thr74‐specific antibody. Thr74 is indeed phosphorylated by MST2, but the efficiency is low, suggesting that MOB1B can activate NDR kinases without the phosphorylation of Thr74. We also showed that the phosphorylated MOB1B activates NDR1 T444D and LATS2 T1041D, in which threonine residues phosphorylated by MST kinases are replaced with phosphorylation‐mimicking aspartic acid, more efficiently than the unphosphorylated MOB1B does. This finding supports that the phosphorylation of MOB1B enhances its ability as a direct activator of NDR kinases.
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