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激活 ezrin 的 F-actin 结合能力:PIP₂ 相互作用和磷酸化的协同作用。

Activation of F-actin binding capacity of ezrin: synergism of PIP₂ interaction and phosphorylation.

机构信息

Institute of Organic and Biomolecular Chemistry, University of Göttingen, Göttingen, Germany.

出版信息

Biophys J. 2011 Apr 6;100(7):1708-17. doi: 10.1016/j.bpj.2011.02.039.

DOI:10.1016/j.bpj.2011.02.039
PMID:21463584
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3072610/
Abstract

Ezrin is a membrane-cytoskeleton linker protein that can bind F-actin in its active conformation. Several means of regulation of ezrin's activity have been described including phosphorylation of Thr-567 and binding of L-α-phosphatidylinositol-4,5-bisphosphate (PIP(2)). However, the relative contributions of these events toward activation of the protein and their potential interdependence are not known. We developed an assay based on solid-supported membranes, to which different ezrin mutants (ezrin T567A (inactive mutant), wild-type, and T567D (active pseudophosphorylated mutant)) were bound, that enabled us to analyze the influence of phosphorylation and PIP(2) binding on ezrin's activation state in vitro. The lipid bilayers employed contained either DOGS-NTA-Ni to bind the proteins via an N-terminal His-tag, or PIP(2), to which ezrin binds via specific binding sites located in the N-terminal region of the protein. Quantitative analysis of the binding behavior of all three proteins to the two different receptor lipids revealed that all three bind with high affinity and specificity to the two receptor lipids. Fluorescence microscopy on ezrin-decorated solid-supported membranes showed that, dependent on the mode of binding and the phosphorylation state, ezrin is capable of binding actin filaments. A clear synergism between phosphorylation and the receptor lipid PIP(2) was observed, suggesting a conformational switch from the dormant to the active, F-actin binding state by recognition of PIP(2), which is enhanced by the phosphorylation.

摘要

埃兹蛋白是一种膜 - 细胞骨架连接蛋白,能够结合 F-肌动蛋白的活性构象。已经描述了几种调节埃兹蛋白活性的方法,包括 Thr-567 的磷酸化和 L-α-磷脂酰肌醇-4,5-二磷酸(PIP(2))的结合。然而,这些事件对蛋白质激活的相对贡献及其潜在的相互依赖性尚不清楚。我们开发了一种基于固体支撑膜的测定法,不同的埃兹蛋白突变体(ezrin T567A(无活性突变体)、野生型和 T567D(活性假磷酸化突变体))可以结合到该膜上,使我们能够分析磷酸化和 PIP(2)结合对 ezrin 体外激活状态的影响。所使用的脂质双层要么包含 DOGS-NTA-Ni 通过 N 端 His 标签结合蛋白,要么包含 PIP(2),通过位于蛋白质 N 端区域的特定结合位点结合 ezrin。对所有三种蛋白质与两种不同受体脂质的结合行为的定量分析表明,所有三种蛋白质都以高亲和力和特异性结合到两种受体脂质上。在 ezrin 修饰的固体支撑膜上进行荧光显微镜观察表明,依赖于结合方式和磷酸化状态,ezrin 能够结合肌动蛋白丝。观察到磷酸化和受体脂质 PIP(2)之间明显的协同作用,表明通过识别 PIP(2)从休眠到活性、与 F-肌动蛋白结合的状态发生构象转换,这种转换通过磷酸化增强。

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High turnover of ezrin T567 phosphorylation: conformation, activity, and cellular function.埃兹蛋白T567磷酸化的高周转率:构象、活性及细胞功能
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