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Monomer–dimer dynamics and distribution of GPI-anchored uPAR are determined by cell surface protein assemblies

机译:GPI锚定的uPAR的单体二聚体动力学和分布取决于细胞表面蛋白装配

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摘要

To search for functional links between glycosylphosphatidylinositol (GPI) protein monomer–oligomer exchange and membrane dynamics and confinement, we studied urokinase plasminogen activator (uPA) receptor (uPAR), a GPI receptor involved in the regulation of cell adhesion, migration, and proliferation. Using a functionally active fluorescent protein–uPAR in live cells, we analyzed the effect that extracellular matrix proteins and uPAR ligands have on uPAR dynamics and dimerization at the cell membrane. Vitronectin directs the recruitment of dimers and slows down the diffusion of the receptors at the basal membrane. The commitment to uPA–plasminogen activator inhibitor type 1–mediated endocytosis and recycling modifies uPAR diffusion and induces an exchange between uPAR monomers and dimers. This exchange is fully reversible. The data demonstrate that cell surface protein assemblies are important in regulating the dynamics and localization of uPAR at the cell membrane and the exchange of monomers and dimers. These results also provide a strong rationale for dynamic studies of GPI-anchored molecules in live cells at steady state and in the absence of cross-linker/clustering agents.
机译:为了寻找糖基磷脂酰肌醇(GPI)蛋白单体-低聚物交换与膜动力学和封闭之间的功能联系,我们研究了尿激酶纤溶酶原激活剂(uPA)受体(uPAR),它是一种参与调节细胞粘附,迁移和增殖的GPI受体。在活细胞中使用功能活跃的荧光蛋白–uPAR,我们分析了细胞外基质蛋白和uPAR配体对uPAR动力学和细胞膜二聚化的影响。玻连蛋白指导二聚体的募集并减慢受体在基膜的扩散。对uPA-纤溶酶原激活物抑制剂1型介导的内吞和再循环的承诺改变了uPAR的扩散,并诱导了uPAR单体与二聚体之间的交换。这种交换是完全可逆的。数据表明,细胞表面蛋白装配对于调节uPAR在细胞膜上的动力学和定位以及单体和二聚体的交换非常重要。这些结果也为在稳态和不存在交联剂/簇剂的情况下在活细胞中动态研究GPI锚定分子提供了有力的依据。

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