Centre de Recherche Université Laval Robert-Giffard, Quebec City, QC, Canada.
Biochemistry. 2010 Jan 12;49(1):166-78. doi: 10.1021/bi901086v.
Cardiac sodium channel Na(v)1.5 plays a critical role in heart excitability and conduction. The molecular mechanism that underlies the expression of Na(v)1.5 at the cell membrane is poorly understood. Previous studies demonstrated that cytoskeleton proteins can be involved in the regulation of cell surface expression and localization of several ion channels. We performed a yeast two-hybrid screen to identify Na(v)1.5-associated proteins that may be involved in channel function and expression. We identified alpha-actinin-2 as an interacting partner of the cytoplasmic loop connecting domains III and IV of Na(v)1.5 (Na(v)1.5/LIII-IV). Co-immunoprecipitation and His(6) pull-down assays confirmed the physical association between Na(v)1.5 and alpha-actinin-2 and showed that the spectrin-like repeat domain is essential for binding of alpha-actinin-2 to Na(v)1.5. Patch-clamp studies revealed that the interaction with alpha-actinin-2 increases sodium channel density without changing their gating properties. Consistent with these findings, coexpression of alpha-actinin-2 and Na(v)1.5 in tsA201 cells led to an increase in the level of expression of Na(v)1.5 at the cell membrane as determined by cell surface biotinylation. Lastly, immunostaining experiments showed that alpha-actinin-2 was colocalized with Na(v)1.5 along the Z-lines and in the plasma membrane. Our data suggest that alpha-actinin-2, which is known to regulate the functional expression of the potassium channels, may play a role in anchoring Na(v)1.5 to the membrane by connecting the channel to the actin cytoskeleton network.
心脏钠离子通道 Na(v)1.5 在心脏兴奋性和传导中起着关键作用。其在细胞膜表达的分子机制尚不清楚。先前的研究表明,细胞骨架蛋白可能参与调节几个离子通道的细胞表面表达和定位。我们进行了酵母双杂交筛选,以鉴定可能参与通道功能和表达的与 Na(v)1.5 相关的蛋白。我们鉴定出α-辅肌动蛋白-2 是连接 Na(v)1.5 的 III 和 IV 结构域的细胞质环的相互作用伙伴 (Na(v)1.5/LIII-IV)。共免疫沉淀和 His(6) 下拉实验证实了 Na(v)1.5 和 α-辅肌动蛋白-2 之间的物理关联,并表明 spectrin 样重复结构域对于 α-辅肌动蛋白-2 与 Na(v)1.5 的结合是必需的。膜片钳研究表明,与 α-辅肌动蛋白-2 的相互作用增加了钠通道的密度,而不改变其门控特性。与这些发现一致的是,在 tsA201 细胞中共表达 α-辅肌动蛋白-2 和 Na(v)1.5 导致细胞膜上 Na(v)1.5 的表达水平增加,这可以通过细胞膜生物素化来确定。最后,免疫染色实验表明,α-辅肌动蛋白-2 与 Na(v)1.5 一起沿 Z 线和质膜共定位。我们的数据表明,α-辅肌动蛋白-2 已知可以调节钾通道的功能性表达,它可能通过将通道连接到肌动蛋白细胞骨架网络来将 Na(v)1.5 锚定在膜上。