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Calcium-dependent dynamics of cadherin interactions at cell–cell junctions

机译:细胞间连接处钙黏着蛋白相互作用的钙依赖性动力学

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摘要

Cadherins play a key role in the dynamics of cell–cell contact formation and remodeling of junctions and tissues. Cadherin–cadherin interactions are gated by extracellular Ca2+, which serves to rigidify the cadherin extracellular domains and promote trans junctional interactions. Here we describe the direct visualization and quantification of spatiotemporal dynamics of N-cadherin interactions across intercellular junctions in living cells using a genetically encodable FRET reporter system. Direct measurements of transjunctional cadherin interactions revealed a sudden, but partial, loss of homophilic interactions (τ = 1.17 ± 0.06 s−1) upon chelation of extracellular Ca2+. A cadherin mutant with reduced adhesive activity (W2A) exhibited a faster, more substantial loss of homophilic interactions (τ = 0.86 ± 0.02 s−1), suggesting two types of native cadherin interactions—one that is rapidly modulated by changes in extracellular Ca2+ and another with relatively stable adhesive activity that is Ca2+ independent. The Ca2+-sensitive dynamics of cadherin interactions were transmitted to the cell interior where β-catenin translocated to N-cadherin at the junction in both cells. These data indicate that cadherins can rapidly convey dynamic information about the extracellular environment to both cells that comprise a junction.
机译:钙黏着蛋白在细胞间接触形成以及连接和组织重塑的动力学中起关键作用。钙黏着蛋白与钙黏着蛋白之间的相互作用受到细胞外Ca 2 + 的控制,该作用可以增强钙黏着蛋白胞外域的结构并促进跨结相互作用。在这里,我们描述了使用可遗传编码的FRET报告系统,在活细胞中跨细胞间连接的N-钙粘着蛋白相互作用的时空动力学的直接可视化和量化。通过直接测量跨结钙粘蛋白的相互作用,发现在细胞外Ca 2 + 螯合后,同源性相互作用突然但部分丧失(τ= 1.17±0.06 s -1 )。粘附活性降低(W2A)的钙粘蛋白突变体表现出更快,更大量的同性相互作用损失(τ= 0.86±0.02 s -1 ),表明两种天然的钙粘蛋白相互作用-一种是快速的可以通过胞外Ca 2 + 的变化来调节,而另一种具有相对稳定的粘附活性的独立于Ca 2 + 的调节。钙粘蛋白相互作用的Ca 2 + 动力学被传递到细胞内部,在这两个细胞的交界处,β-catenin易位至N-cadherin。这些数据表明钙粘着蛋白可以将有关细胞外环境的动态信息迅速传达给组成连接的两个细胞。

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