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雄激素受体的磷酸化和活性受与蛋白磷酸酶1的结合调控。

Androgen receptor phosphorylation and activity are regulated by an association with protein phosphatase 1.

作者信息

Chen Shaoyong, Kesler Cristina T, Paschal Bryce M, Balk Steven P

机构信息

Cancer Biology Program, Hematology-Oncology Division, Department of Medicine, Beth Israel Deaconess Medical Center, Harvard Medical School, Boston, Massachusetts 02215, USA.

出版信息

J Biol Chem. 2009 Sep 18;284(38):25576-84. doi: 10.1074/jbc.M109.043133. Epub 2009 Jul 21.

Abstract

Androgen receptor (AR) is phosphorylated at multiple sites in response to ligand binding, but the functional consequences and mechanisms regulating AR phosphorylation remain to be established. We observed initially that okadaic acid, an inhibitor of the major PPP family serine/threonine phosphatases PP2A and protein phosphatase 1 (PP1), had cell type-dependent effects on AR expression. More specific inhibitors of PP2A (fostriecin) and PP1 (tautomycin and siRNA against the PP1alpha catalytic subunit) demonstrated that PP1 and protein phosphatase 2A had opposite effects on AR protein and transcriptional activity. PP1 inhibition enhanced proteasome-mediated AR degradation, while PP1alpha overexpression increased AR expression and markedly enhanced AR transcriptional activity. Coprecipitation experiments demonstrated an AR-PP1 interaction, while immunofluorescence and nuclear-cytoplasmic fractionation showed androgen-stimulated nuclear translocation of both AR and PP1 in prostate cancer cells. Studies with phosphospecific AR antibodies showed that PP1 inhibition dramatically increased phosphorylation of Ser-650, a site in the AR hinge region shown to mediate nuclear export. Significantly, PP1 inhibition caused a marked decrease in nuclear localization of the wild-type AR, but did not alter total or nuclear levels of a S650A mutant AR. These findings reveal a critical role of PP1 in regulating AR protein stability and nuclear localization through dephosphorylation of Ser-650. Moreover, AR may function as a PP1 regulatory subunit and mediate PP1 recruitment to chromatin, where it can modulate transcription and splicing.

摘要

雄激素受体(AR)在配体结合后会在多个位点发生磷酸化,但其功能后果以及调节AR磷酸化的机制仍有待确定。我们最初观察到,冈田酸(一种主要的PPP家族丝氨酸/苏氨酸磷酸酶PP2A和蛋白磷酸酶1(PP1)的抑制剂)对AR表达具有细胞类型依赖性影响。PP2A(福司曲星)和PP1( tautomycin以及针对PP1α催化亚基的小干扰RNA)的更特异性抑制剂表明,PP1和蛋白磷酸酶2A对AR蛋白和转录活性具有相反的作用。抑制PP1可增强蛋白酶体介导的AR降解,而PP1α过表达则增加AR表达并显著增强AR转录活性。共沉淀实验证明了AR与PP1之间存在相互作用,而免疫荧光和核质分级分离显示,在前列腺癌细胞中,雄激素刺激了AR和PP1的核转位。使用磷酸特异性AR抗体进行的研究表明,抑制PP1会显著增加Ser-650的磷酸化,该位点位于AR铰链区,已证明可介导核输出。重要的是,抑制PP1会导致野生型AR的核定位显著降低,但不会改变S650A突变型AR的总量或核水平。这些发现揭示了PP1在通过去磷酸化Ser-650来调节AR蛋白稳定性和核定位方面的关键作用。此外,AR可能作为PP1的调节亚基发挥作用,并介导PP1募集到染色质,在那里它可以调节转录和剪接。

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