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埃兹蛋白激活过程中磷酸化诱导的可塑性变化的单分子检测。

Single-molecule detection of phosphorylation-induced plasticity changes during ezrin activation.

作者信息

Liu Dan, Ge Ling, Wang Fengsong, Takahashi Hirohide, Wang Dongmei, Guo Zhen, Yoshimura Shige H, Ward Tarsha, Ding Xia, Takeyasu Kunio, Yao Xuebiao

机构信息

Division of Cellular Dynamics, Hefei National Laboratory for Physical Sciences, Hefei 230027, China.

出版信息

FEBS Lett. 2007 Jul 24;581(18):3563-71. doi: 10.1016/j.febslet.2007.06.071. Epub 2007 Jul 3.

DOI:10.1016/j.febslet.2007.06.071
PMID:17628548
Abstract

Ezrin-radixin-moesin protein family provides a regulated link between the cortical actin cytoskeleton and the plasma membrane. Phosphorylation of ezrin has been functionally linked to membrane dynamics and plasticity. Our recent study demonstrated that phosphorylation of the conserved T567 residue of ezrin alters the physiology of gastric parietal cells. However, the molecular mechanism of phosphorylation-induced ezrin activation has remained elusive. Here we use atomic force microscopy (AFM) to probe phosphorylation-mediated activation of ezrin in single molecules. The phospho-mimicking and non-phosphorylatable mutant ezrin proteins were generated and purified to homogeneity. Comparative analyses of two ezrin mutants by AFM demonstrate the unfolding of the N- and C-terminal domains upon the phospho-activation. To measure the physical force underlying the inter-domain contact during mechanical unfolding, we probed the defined region of ezrin using the N-terminal ezrin coated onto the AFM tip. Comparative force measurements indicate that T567 phosphorylation-induced unfolding of ezrin favors the inter-molecular association. Taken together, these results provide molecular illustration of phosphorylation elicited functional activation of ERM proteins and indicate that stimulus-induced protein conformational change can be used as a signaling mechanism orchestrating cellular dynamics.

摘要

埃兹蛋白-根蛋白-膜突蛋白家族在皮质肌动蛋白细胞骨架和质膜之间提供了一种受调控的连接。埃兹蛋白的磷酸化在功能上与膜动力学和可塑性相关。我们最近的研究表明,埃兹蛋白保守的T567残基的磷酸化改变了胃壁细胞的生理功能。然而,磷酸化诱导的埃兹蛋白激活的分子机制仍然不清楚。在这里,我们使用原子力显微镜(AFM)来探测单分子中磷酸化介导的埃兹蛋白激活。生成并纯化了模拟磷酸化和不可磷酸化的埃兹蛋白突变体,使其达到同质状态。通过AFM对两种埃兹蛋白突变体进行比较分析,结果表明磷酸化激活后N端和C端结构域发生了解折叠。为了测量机械解折叠过程中结构域间接触的物理力,我们使用涂覆在AFM尖端的埃兹蛋白N端来探测埃兹蛋白的特定区域。比较力测量结果表明,T5…

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