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Expression of GIV/Girdin, a metastasis-related protein, predicts patient survival in colon cancer.GIV/Girdin 表达,一种转移相关蛋白,预测结肠癌患者的生存。
FASEB J. 2011 Feb;25(2):590-9. doi: 10.1096/fj.10-167304. Epub 2010 Oct 25.
2
Regulators of G protein signaling proteins as targets for drug discovery.G 蛋白信号转导调节蛋白作为药物发现的靶点。
Prog Mol Biol Transl Sci. 2010;91:81-119. doi: 10.1016/S1877-1173(10)91004-1.
3
Nucleobindin 1 is a calcium-regulated guanine nucleotide dissociation inhibitor of G{alpha}i1.核结合蛋白 1 是一种钙调节鸟嘌呤核苷酸解离抑制剂,可抑制 Gαi1。
J Biol Chem. 2010 Oct 8;285(41):31647-60. doi: 10.1074/jbc.M110.148429. Epub 2010 Aug 2.
4
Networking with AKAPs: context-dependent regulation of anchored enzymes.与A激酶锚定蛋白相互作用:锚定酶的上下文依赖性调节
Mol Interv. 2010 Apr;10(2):86-97. doi: 10.1124/mi.10.2.6.
5
A structural determinant that renders G alpha(i) sensitive to activation by GIV/girdin is required to promote cell migration.一个使 Gαi 对 GIV/girdin 的激活敏感的结构决定因素对于促进细胞迁移是必需的。
J Biol Chem. 2010 Apr 23;285(17):12765-77. doi: 10.1074/jbc.M109.045161. Epub 2010 Feb 15.
6
Girding for migratory cues: roles of the Akt substrate Girdin in cancer progression and angiogenesis.为迁徙线索做准备:Akt 底物 Girdin 在癌症进展和血管生成中的作用。
Cancer Sci. 2010 Apr;101(4):836-42. doi: 10.1111/j.1349-7006.2009.01487.x. Epub 2010 Feb 2.
7
Revised role of glycosaminoglycans in TAT protein transduction domain-mediated cellular transduction.糖胺聚糖在 TAT 蛋白转导结构域介导的细胞转导中的修正作用。
J Biol Chem. 2010 Jan 8;285(2):1500-7. doi: 10.1074/jbc.M109.021964. Epub 2009 Oct 26.
8
Calnuc plays a role in dynamic distribution of Galphai but not Gbeta subunits and modulates ACTH secretion in AtT-20 neuroendocrine secretory cells.Calnuc 参与 Galphai 但不参与 Gbeta 亚基的动态分布,并调节 AtT-20 神经内分泌分泌细胞中的 ACTH 分泌。
Mol Neurodegener. 2009 Mar 25;4:15. doi: 10.1186/1750-1326-4-15.
9
GIV is a nonreceptor GEF for G alpha i with a unique motif that regulates Akt signaling.GIV是一种针对Gαi的非受体鸟苷酸交换因子,具有调控Akt信号传导的独特基序。
Proc Natl Acad Sci U S A. 2009 Mar 3;106(9):3178-83. doi: 10.1073/pnas.0900294106. Epub 2009 Feb 11.
10
Activation of Galphai3 triggers cell migration via regulation of GIV.Gαi3的激活通过调控GIV触发细胞迁移。
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Calnuc(核钙黏蛋白 1)和 NUCB2(核钙黏蛋白 2)上的 G 蛋白结合位点定义了一类新的 G(alpha)i 调节基序。

G Protein binding sites on Calnuc (nucleobindin 1) and NUCB2 (nucleobindin 2) define a new class of G(alpha)i-regulatory motifs.

机构信息

Department of Cellular and Molecular Medicine, University of California, San Diego,La Jolla, California 92093, USA.

出版信息

J Biol Chem. 2011 Aug 12;286(32):28138-49. doi: 10.1074/jbc.M110.204099. Epub 2011 Jun 8.

DOI:10.1074/jbc.M110.204099
PMID:21653697
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3151059/
Abstract

Heterotrimeric G proteins are molecular switches modulated by families of structurally and functionally related regulators. GIV (Gα-interacting vesicle-associated protein) is the first non-receptor guanine nucleotide exchange factor (GEF) that activates Gα(i) subunits via a defined, evolutionarily conserved motif. Here we found that Calnuc and NUCB2, two highly homologous calcium-binding proteins, share a common motif with GIV for Gα(i) binding and activation. Bioinformatics searches and structural analysis revealed that Calnuc and NUCB2 possess an evolutionarily conserved motif with sequence and structural similarity to the GEF sequence of GIV. Using in vitro pulldown and competition assays, we demonstrate that this motif binds preferentially to the inactive conformation of Gα(i1) and Gα(i3) over other Gα subunits and, like GIV, docks onto the α3/switch II cleft. Calnuc binding was impaired when Lys-248 in the α3 helix of Gα(i3) was replaced with M, the corresponding residue in Gα(o), which does not bind to Calnuc. Moreover, mutation of hydrophobic residues in the conserved motif predicted to dock on the α3/switch II cleft of Gα(i3) impaired the ability of Calnuc and NUCB2 to bind and activate Gα(i3) in vitro. We also provide evidence that calcium binding to Calnuc and NUCB2 abolishes their interaction with Gα(i3) in vitro and in cells, probably by inducing a conformational change that renders the Gα(i)-binding residues inaccessible. Taken together, our results identify a new type of Gα(i)-regulatory motif named the GBA motif (for Gα-binding and -activating motif), which is conserved across different proteins throughout evolution. These findings provide the structural basis for the properties of Calnuc and NUCB2 binding to Gα subunits and its regulation by calcium ions.

摘要

三聚体 G 蛋白是受结构和功能相关调节剂家族调控的分子开关。GIV(与 Gα 相互作用的囊泡相关蛋白)是第一个通过定义明确的、进化上保守的基序激活 Gα(i)亚基的非受体鸟嘌呤核苷酸交换因子 (GEF)。在这里,我们发现 Calnuc 和 NUCB2 这两种高度同源的钙结合蛋白与 GIV 具有共同的基序,用于 Gα(i)结合和激活。生物信息学搜索和结构分析表明,Calnuc 和 NUCB2 具有与 GIV 的 GEF 序列具有序列和结构相似性的进化上保守的基序。通过体外下拉和竞争测定,我们证明该基序优先结合 Gα(i1)和 Gα(i3)的无活性构象,而不是其他 Gα 亚基,并且与 GIV 一样,停靠在 α3/开关 II 裂隙上。当 Gα(i3)α3 螺旋中的 Lys-248 被替换为 Gα(o)中的相应残基 M 时,Calnuc 的结合受到损害,而 Gα(o)不与 Calnuc 结合。此外,预测与 Gα(i3)的 α3/开关 II 裂隙结合的保守基序中的疏水残基的突变削弱了 Calnuc 和 NUCB2 在体外结合和激活 Gα(i3)的能力。我们还提供了证据表明,钙结合到 Calnuc 和 NUCB2 会在体外和细胞中破坏它们与 Gα(i3)的相互作用,可能是通过诱导构象变化使 Gα(i)-结合残基无法接近。总之,我们的结果确定了一种新的 Gα(i)-调节基序,称为 GBA 基序(用于 Gα 结合和激活基序),该基序在整个进化过程中在不同的蛋白质中是保守的。这些发现为 Calnuc 和 NUCB2 与 Gα 亚基结合及其受钙离子调节的特性提供了结构基础。