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交叉相关波动分析揭示了新形成黏着点中磷酸化调节的桩蛋白-FAK 复合物。

Cross-correlated fluctuation analysis reveals phosphorylation-regulated paxillin-FAK complexes in nascent adhesions.

机构信息

Department of Cell Biology, University of Virginia, Charlottesville, Virginia.

Department of Cell Biology, University of Virginia, Charlottesville, Virginia.

出版信息

Biophys J. 2011 Feb 2;100(3):583-592. doi: 10.1016/j.bpj.2010.12.3719.

Abstract

We used correlation methods to detect and quantify interactions between paxillin and focal adhesion kinase (FAK) in migrating cells. Cross-correlation raster-scan image correlation spectroscopy revealed that wild-type paxillin and the phosphorylation-inhibiting paxillin mutant Y31F-Y118F do not interact with FAK in the cytosol but a phosphomimetic mutant of paxillin, Y31E-Y118E, does. By extending cross-correlation number and brightness analysis to the total internal reflection fluorescence modality, we were able to show that tetramers of paxillin and FAK form complexes in nascent adhesions with a 1:1 stoichiometry ratio. The phosphomimetic mutations on paxillin increase the size of the complex and the assembly rate of nascent adhesions, suggesting that the physical molecular aggregation of paxillin and FAK regulates adhesion formation. In contrast, when phosphorylation is inhibited, the interaction decreases and the adhesions tend to elongate rather than turn over. These direct in vivo data show that the phosphorylation of paxillin is specific to adhesions and leads to localized complex formation with FAK to regulate the dynamics of nascent adhesions.

摘要

我们使用相关方法来检测和量化在迁移细胞中粘着斑激酶(FAK)与桩蛋白(paxillin)之间的相互作用。互相关联的光栅扫描图像相关光谱学揭示,野生型的桩蛋白和磷酸化抑制突变体 Y31F-Y118F 不会与细胞质中的 FAK 相互作用,但磷酸化模拟突变体 Y31E-Y118E 则会。通过将互相关数和亮度分析扩展到全内反射荧光模式,我们能够表明,桩蛋白和 FAK 的四聚体以 1:1 的化学计量比形成在新生黏附物中的复合物。桩蛋白上的磷酸化模拟突变增加了复合物的大小和新生黏附物的组装速率,表明 paxillin 和 FAK 的物理分子聚集调节黏附的形成。相比之下,当磷酸化被抑制时,相互作用减少,黏附物倾向于延伸而不是翻转。这些直接的体内数据表明,paxillin 的磷酸化是特异于黏附物的,并导致与 FAK 的局部复合物形成,从而调节新生黏附物的动力学。

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