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Rapid internalization and surface expression of a functional fluorescently tagged G-protein-coupled glutamate receptor.

机译:功能性的荧光标记的G蛋白偶联的谷氨酸受体的快速内在化和表面表达。

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摘要

l-Glutamate is the principal excitatory neurotransmitter in the vertebrate central nervous system, where it mediates many of its actions via G-protein-coupled metabotropic glutamate (mGlu) receptors. Since little is known about the dynamics of mGlu receptors at the plasma membrane, we have constructed a fusion protein comprising the mGlu receptor subtype 1alpha (mGlu1alpha) and green fluorescent protein (GFP). Using imaging of Ca2+ release from intracellular stores as a functional assay, the agonist pharmacology of this fluorescently tagged receptor was found to be similar to that of the wild-type receptor when expressed in HEK-293 cells. Receptor movement and function were measured simultaneously by combined imaging of Ca2+, using fura-red, and GFP fluorescence in single cells. Exposure to agonist induced a rapid loss of up to 30% of membrane-associated fluorescence, with a corresponding decrease in the functional response. Following removal of the agonist there was recovery of both the membrane fluorescence and the functional response. These data suggest that the surface expression of G-protein-coupled glutamate receptors might be rapidly regulated in response to agonist activation.
机译:谷氨酸是脊椎动物中枢神经系统的主要兴奋性神经递质,它通过G蛋白偶联的代谢型谷氨酸(mGlu)受体介导其许多作用。由于对质膜上mGlu受体的动力学知之甚少,我们构建了一种融合蛋白,该蛋白包含mGlu受体亚型1alpha(mGlu1alpha)和绿色荧光蛋白(GFP)。使用从细胞内存储中释放的Ca2 +的成像作为功能分析,发现该荧光标记受体的激动剂药理学与在HEK-293细胞中表达的野生型受体相似。通过对呋喃红和GFP荧光在单个细胞中的Ca2 +进行联合成像,同时测量受体的运动和功能。暴露于激动剂会引起多达30%的膜相关荧光迅速丧失,相应的功能反应也会降低。除去激动剂后,膜荧光和功能响应均恢复。这些数据表明,G蛋白偶联的谷氨酸受体的表面表达可能会受激动剂激活而快速调节。

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