Leontiadis Leonidas J, Papakonstantinou Maria P, Georgoussi Zafiroula
Laboratory of Cellular Signaling and Molecular Pharmacology, Institute of Biology, National Center for Scientific Research Demokritos, Ag. Paraskevi-Attikis, Athens, Greece.
Cell Signal. 2009 Jul;21(7):1218-28. doi: 10.1016/j.cellsig.2009.03.013. Epub 2009 Mar 24.
In vitro studies have shown that the Regulator of G protein Signaling 4 (RGS4) interacts with the C-termini of mu- and delta-opioid receptors (mu-OR, delta-OR) (Georgoussi et al., 2006, Cell. Signal.18, 771-782). Herein we demonstrate that RGS4 associates with these receptors in living cells and forms selective complexes with Gi/Go proteins in a receptor dependent manner. This interaction occurs within the predicted fourth intracellular loop of mu, delta-ORs as part of a signaling complex consisting of the opioid receptor, activated Galpha and RGS4. RGS4 is recruited to the plasma membrane upon opioid receptor stimulation. Expression of RGS4 in HEK293 cells attenuated agonist-mediated extracellular signal regulated kinase (ERK1,2) phosphorylation for both receptors and accelerated agonist-induced internalization of the delta-OR. RGS4 lacking its N-terminal domain failed to interact with both opioid receptors and to modulate opioid receptor signaling. Our findings demonstrate that RGS4 plays a key role in G protein coupling selectivity and signaling of the mu- and delta-OmicronRs.
体外研究表明,G蛋白信号调节因子4(RGS4)与μ-阿片受体和δ-阿片受体(μ-OR、δ-OR)的C末端相互作用(Georgoussi等人,2006年,《细胞信号》18卷,771 - 782页)。在此我们证明,RGS4在活细胞中与这些受体相关联,并以受体依赖的方式与Gi/Go蛋白形成选择性复合物。这种相互作用发生在μ-OR、δ-OR预测的第四个细胞内环内,是由阿片受体、活化的Gα和RGS4组成的信号复合物的一部分。阿片受体受刺激后,RGS4被募集到质膜。RGS4在HEK293细胞中的表达减弱了两种受体激动剂介导的细胞外信号调节激酶(ERK1,2)磷酸化,并加速了激动剂诱导的δ-OR内化。缺少N末端结构域的RGS4无法与两种阿片受体相互作用,也无法调节阿片受体信号传导。我们的研究结果表明,RGS4在μ-和δ-阿片受体的G蛋白偶联选择性和信号传导中起关键作用。
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