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二价阳离子以不同方式调节整合素αIIb胞质尾与β3以及与钙和整合素结合蛋白的结合。

Divalent cations differentially regulate integrin alphaIIb cytoplasmic tail binding to beta3 and to calcium- and integrin-binding protein.

作者信息

Vallar L, Melchior C, Plançon S, Drobecq H, Lippens G, Regnault V, Kieffer N

机构信息

Laboratoire Franco-Luxembourgeois de Recherche Biomédicale (CNRS and CRP-Santé), Centre Universitaire, L-1511 Luxembourg, Grand Duchy of Luxembourg.

出版信息

J Biol Chem. 1999 Jun 11;274(24):17257-66. doi: 10.1074/jbc.274.24.17257.

DOI:10.1074/jbc.274.24.17257
PMID:10358085
Abstract

We have used recombinant or synthetic alphaIIb and beta3 integrin cytoplasmic peptides to study their in vitro complexation and ligand binding capacity by surface plasmon resonance. alpha.beta heterodimerization occurred in a 1:1 stoichiometry with a weak KD in the micromolar range. Divalent cations were not required for this association but stabilized the alpha.beta complex by decreasing the dissociation rate. alpha.beta complexation was impaired by the R995A substitution or the KVGFFKR deletion in alphaIIb but not by the beta3 S752P mutation. Recombinant calcium- and integrin-binding protein (CIB), an alphaIIb-specific ligand, bound to the alphaIIb cytoplasmic peptide in a Ca2+- or Mn2+-independent, one-to-one reaction with a KD value of 12 microM. In contrast, in vitro liquid phase binding of CIB to intact alphaIIbbeta3 occurred preferentially with Mn2+-activated alphaIIbbeta3 conformers, as demonstrated by enhanced coimmunoprecipitation of CIB with PAC-1-captured Mn2+-activated alphaIIbbeta3, suggesting that Mn2+ activation of intact alphaIIbbeta3 induces the exposure of a CIB-binding site, spontaneously exposed by the free alphaIIb peptide. Since CIB did not stimulate PAC-1 binding to inactive alphaIIbbeta3 nor prevented activated alphaIIbbeta3 occupancy by PAC-1, we conclude that CIB does not regulate alphaIIbbeta3 inside-out signaling, but rather is involved in an alphaIIbbeta3 post-receptor occupancy event.

摘要

我们使用重组或合成的αIIb和β3整合素细胞质肽,通过表面等离子体共振研究它们的体外复合和配体结合能力。αβ异二聚化以1:1的化学计量比发生,解离常数(KD)在微摩尔范围内较弱。这种结合不需要二价阳离子,但通过降低解离速率来稳定αβ复合物。αIIb中的R995A取代或KVGFFKR缺失会损害αβ复合,但β3 S752P突变则不会。重组钙和整合素结合蛋白(CIB)是一种αIIb特异性配体,以与KD值为12微摩尔的Ca2+或Mn2+无关的一对一反应结合到αIIb细胞质肽上。相比之下,如CIB与PAC-1捕获的Mn2+激活的αIIbbeta3的共免疫沉淀增强所证明的,CIB与完整的αIIbbeta3的体外液相结合优先发生在Mn2+激活的αIIbbeta3构象体上,这表明完整的αIIbbeta3的Mn2+激活诱导了一个CIB结合位点的暴露,该位点由游离的αIIb肽自发暴露。由于CIB既不刺激PAC-1与无活性的αIIbbeta3结合,也不阻止PAC-1占据激活的αIIbbeta3,我们得出结论,CIB不调节αIIbbeta3的外向内信号传导,而是参与αIIbbeta3受体后占据事件。

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