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NIPP-1对核蛋白磷酸酶-1调控的分子决定因素

Molecular determinants of nuclear protein phosphatase-1 regulation by NIPP-1.

作者信息

Beullens M, Van Eynde A, Vulsteke V, Connor J, Shenolikar S, Stalmans W, Bollen M

机构信息

Afdeling Biochemie, Faculteit Geneeskunde, Katholieke Universiteit Leuven, B-3000 Leuven, Belgium.

出版信息

J Biol Chem. 1999 May 14;274(20):14053-61. doi: 10.1074/jbc.274.20.14053.

DOI:10.1074/jbc.274.20.14053
PMID:10318819
Abstract

NIPP-1 is a subunit of the major nuclear protein phosphatase-1 (PP-1) in mammalian cells and potently inhibits PP-1 activity in vitro. Using yeast two-hybrid and co-sedimentation assays, we mapped a PP-1-binding site and the inhibition function to the central one-third domain of NIPP-1. Full-length NIPP-1 (351 residues) and the central domain, NIPP-1(143-217), were equally potent PP-1 inhibitors (IC50 = 0.3 nM). Synthetic peptides spanning the central domain of NIPP-1 further narrowed the PP-1 inhibitory function to residues 191-200. A second, noninhibitory PP-1-binding site was identified by far-Western assays with digoxygenin-conjugated catalytic subunit (PP-1C) and included a consensus RVXF motif (residues 200-203) found in many other PP-1-binding proteins. The substitutions, V201A and/or F203A, in the RVXF motif, or phosphorylation of Ser199 or Ser204, which are established phosphorylation sites for protein kinase A and protein kinase CK2, respectively, prevented PP-1C-binding by NIPP-1(191-210) in the far-Western assay. NIPP-1(191-210) competed for PP-1 inhibition by full-length NIPP-1(1-351), inhibitor-1 and inhibitor-2, and dissociated PP-1C from inhibitor-1- and NIPP-1(143-217)-Sepharose but not from full-length NIPP-1(1-351)-Sepharose. Together, these data identified some of the key elements in the central domain of NIPP-1 that regulate PP-1 activity and suggested that the flanking sequences stabilize the association of NIPP-1 with PP-1C.

摘要

NIPP-1是哺乳动物细胞中主要核蛋白磷酸酶-1(PP-1)的一个亚基,在体外能有效抑制PP-1的活性。利用酵母双杂交和共沉降分析,我们将PP-1结合位点和抑制功能定位到NIPP-1的中央三分之一结构域。全长NIPP-1(351个氨基酸残基)和中央结构域NIPP-1(143 - 217)是同等有效的PP-1抑制剂(IC50 = 0.3 nM)。跨越NIPP-1中央结构域的合成肽进一步将PP-1抑制功能缩小到191 - 200位氨基酸残基。通过用洋地黄毒苷偶联的催化亚基(PP-1C)进行远缘Western分析鉴定出第二个非抑制性PP-1结合位点,其中包括许多其他PP-1结合蛋白中发现的共有RVXF基序(200 - 203位氨基酸残基)。RVXF基序中的V201A和/或F203A替换,或Ser199或Ser204的磷酸化(分别是蛋白激酶A和蛋白激酶CK2的既定磷酸化位点),在远缘Western分析中阻止了NIPP-1(191 - 210)与PP-1C的结合。NIPP-1(191 - 210)竞争全长NIPP-1(1 - 351)、抑制剂-1和抑制剂-2对PP-1的抑制作用,并使PP-1C从抑制剂-1和NIPP-1(143 - 217)-琼脂糖凝胶上解离,但不能从全长NIPP-1(1 - 351)-琼脂糖凝胶上解离。总之,这些数据确定了NIPP-1中央结构域中调节PP-1活性的一些关键元件,并表明侧翼序列稳定了NIPP-1与PP-1C的结合。

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