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钙敏感受体的激活促使紧密连接蛋白在细胞顶膜的沉积。

Activation of the Ca²+-sensing receptor induces deposition of tight junction components to the epithelial cell plasma membrane.

机构信息

Department of Cellular and Molecular Physiology, Yale School of Medicine, New Haven, CT 06520, USA.

出版信息

J Cell Sci. 2013 Nov 15;126(Pt 22):5132-42. doi: 10.1242/jcs.127555. Epub 2013 Sep 6.

Abstract

The Ca(2+)-sensing receptor (CaSR) belongs to the G-protein-coupled receptor superfamily and plays essential roles in divalent ion homeostasis and cell differentiation. Because extracellular Ca(2+) is essential for the development of stable epithelial tight junctions (TJs), we hypothesized that the CaSR participates in regulating TJ assembly. We first assessed the expression of the CaSR in Madin-Darby canine kidney (MDCK) cells at steady state and following manipulations that modulate TJ assembly. Next, we examined the effects of CaSR agonists and antagonists on TJ assembly. Immunofluorescence studies indicate that endogenous CaSR is located at the basolateral pole of MDCK cells. Stable transfection of human CaSR in MDCK cells further reveals that this protein co-distributes with β-catenin on the basolateral membrane. Switching MDCK cells from low-Ca(2+) medium to medium containing a normal Ca(2+) concentration significantly increases CaSR expression at both the mRNA and protein levels. Exposure of MDCK cells maintained in low-Ca(2+) conditions to the CaSR agonists neomycin, Gd(3+) or R-568 causes the transient relocation of the tight junction components ZO-1 and occludin to sites of cell-cell contact, while inducing no significant changes in the expression of mRNAs encoding junction-associated proteins. Stimulation of CaSR also increases the interaction between ZO-1 and the F-actin-binding protein I-afadin. This effect does not involve activation of the AMP-activated protein kinase. By contrast, CaSR inhibition by NPS-2143 significantly decreases interaction of ZO-1 with I-afadin and reduces deposition of ZO-1 at the cell surface following a Ca(2+) switch from 5 µM to 200 µM [Ca(2+)]e. Pre-exposure of MDCK cells to the cell-permeant Ca(2+) chelator BAPTA-AM, similarly prevents TJ assembly caused by CaSR activation. Finally, stable transfection of MDCK cells with a cDNA encoding a human disease-associated gain-of-function mutant form of the CaSR increases the transepithelial electrical resistance of these cells in comparison to expression of the wild-type human CaSR. These observations suggest that the CaSR participates in regulating TJ assembly.

摘要

钙敏感受体 (CaSR) 属于 G 蛋白偶联受体超家族,在二价离子稳态和细胞分化中发挥重要作用。由于细胞外 Ca2+ 对于稳定上皮细胞紧密连接 (TJ) 的形成至关重要,我们假设 CaSR 参与调节 TJ 的组装。我们首先评估了 CaSR 在稳定状态下以及调节 TJ 组装的操作后在 Madin-Darby 犬肾 (MDCK) 细胞中的表达。接下来,我们研究了 CaSR 激动剂和拮抗剂对 TJ 组装的影响。免疫荧光研究表明,内源性 CaSR 位于 MDCK 细胞的基底外侧极。在 MDCK 细胞中稳定转染人 CaSR 进一步表明,这种蛋白与 β-连环蛋白共分布在基底外侧膜上。将 MDCK 细胞从低钙培养基切换到含有正常钙浓度的培养基中,可显著增加 CaSR 在 mRNA 和蛋白质水平的表达。将在低钙条件下维持的 MDCK 细胞暴露于 CaSR 激动剂新霉素、Gd(3+)或 R-568 会导致紧密连接成分 ZO-1 和 occludin 瞬时重新定位到细胞-细胞接触部位,而不会引起与连接相关蛋白编码 mRNA 的表达发生显著变化。CaSR 的刺激还增加了 ZO-1 与 F-肌动蛋白结合蛋白 I-afadin 的相互作用。这种效应不涉及 AMP 激活蛋白激酶的激活。相比之下,CaSR 抑制物 NPS-2143 显著降低了 ZO-1 与 I-afadin 的相互作用,并在 Ca2+ 从 5 µM 切换到 200 µM [Ca2+]e 后减少 ZO-1 在细胞表面的沉积。预先将 MDCK 细胞暴露于细胞通透钙螯合剂 BAPTA-AM 同样可以防止 CaSR 激活引起的 TJ 组装。最后,与表达野生型人 CaSR 相比,用编码人疾病相关功能获得性突变形式的 CaSR 的 cDNA 稳定转染 MDCK 细胞会增加这些细胞的跨上皮电阻。这些观察结果表明 CaSR 参与调节 TJ 的组装。

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