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通过激活GPER抑制储存式钙内流:对内皮细胞钙信号钳制作用的贡献。

Suppression of store-operated Ca entry by activation of GPER: contribution to a clamping effect on endothelial Ca signaling.

作者信息

Terry Lara E, VerMeer Mark, Giles Jennifer, Tran Quang-Kim

机构信息

Department of Physiology and Pharmacology, Des Moines University Osteopathic Medical Center, 3200 Grand Avenue, Des Moines, IA 50312, U.S.A.

出版信息

Biochem J. 2017 Oct 23;474(21):3627-3642. doi: 10.1042/BCJ20170630.

DOI:10.1042/BCJ20170630
PMID:28935720
Abstract

The G protein-coupled estrogen receptor 1 (GPER, formerly also known as GPR30) modulates many Ca-dependent activities in endothelial cells. However, the underlying mechanisms are poorly understood. We recently reported that GPER acts to prolong cytoplasmic Ca signals by interacting with and promoting inhibitory phosphorylation of the plasma membrane Ca-ATPase. In the present study, we examined the role of GPER activation in modulating store-operated Ca entry (SOCE) via effects on the stromal interaction molecule 1 (STIM1). GPER activation by agonist G-1 reduces the peak but prolongs the plateau of bradykinin-induced Ca signals in primary endothelial cells. G-1 dose-dependently inhibits thapsigargin-induced SOCE measured by the Mn quenching method. GPER heterologous expression reduces SOCE, which is further pronounced by G-1 treatment. Consistently, GPER gene silencing in endothelial cells is associated with an increase in SOCE. Treatment with G-1 reduces puncta formation by STIM1 triggered by the activation of SOCE. The effect of GPER activation to inhibit SOCE is not affected by combined nonphosphorylatable substitutions at serines 486 and 668 on STIM1, but is substantially reduced by similar substitutions at serines 575, 608 and 621. Taken together with our recently reported inhibitory actions of GPER on Ca efflux, the current data contribute to a model in which GPER acts to clamp agonist-induced cytoplasmic Ca signals. Kinetic modeling based on current and reported data is used to estimate the overall effect of GPER activation on point activity of endothelial nitric oxide synthase during the time course of agonist-induced total Ca signals.

摘要

G蛋白偶联雌激素受体1(GPER,以前也称为GPR30)调节内皮细胞中许多依赖钙的活动。然而,其潜在机制尚不清楚。我们最近报道,GPER通过与质膜钙ATP酶相互作用并促进其抑制性磷酸化来延长细胞质钙信号。在本研究中,我们研究了GPER激活通过对基质相互作用分子1(STIM1)的影响来调节钙库操纵性钙内流(SOCE)的作用。激动剂G-1激活GPER可降低原发性内皮细胞中缓激肽诱导的钙信号峰值,但延长其平台期。G-1以剂量依赖性方式抑制毒胡萝卜素诱导的SOCE(通过锰淬灭法测量)。GPER异源表达降低SOCE,G-1处理可进一步增强这种作用。一致地,内皮细胞中GPER基因沉默与SOCE增加有关。用G-1处理可减少由SOCE激活触发的STIM1点状形成。GPER激活抑制SOCE的作用不受STIM1丝氨酸486和668处联合非磷酸化替代的影响,但在丝氨酸575、608和621处进行类似替代时,该作用会显著降低。结合我们最近报道的GPER对钙外流的抑制作用,目前的数据有助于建立一个模型,其中GPER起到钳制激动剂诱导的细胞质钙信号的作用。基于当前和已报道数据的动力学建模用于估计在激动剂诱导的总钙信号时间过程中,GPER激活对内皮型一氧化氮合酶点活性的总体影响。

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