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High-Resolution Quantitative Immunogold Analysis of Membrane Receptors at Retinal Ribbon Synapses

机译:视网膜丝带突触的膜受体的高分辨率定量免疫金分析。

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摘要

Retinal ganglion cells (RGCs) receive excitatory glutamatergic input from bipolar cells. Synaptic excitation of RGCs is mediated postsynaptically by NMDA receptors (NMDARs) and AMPA receptors (AMPARs). Physiological data have indicated that glutamate receptors at RGCs are expressed not only in postsynaptic but also in perisynaptic or extrasynaptic membrane compartments. However, precise anatomical locations for glutamate receptors at RGC synapses have not been determined. Although a high-resolution quantitative analysis of glutamate receptors at central synapses is widely employed, this approach has had only limited success in the retina. We developed a postembedding immunogold method for analysis of membrane receptors, making it possible to estimate the number, density and variability of these receptors at retinal ribbon synapses. Here we describe the tools, reagents, and the practical steps that are needed for: 1) successful preparation of retinal fixation, 2) freeze-substitution, 3) postembedding immunogold electron microscope (EM) immunocytochemistry and, 4) quantitative visualization of glutamate receptors at ribbon synapses.
机译:视网膜神经节细胞(RGC)从双极细胞接受兴奋性谷氨酸能输入。 RGC的突触激发是由NMDA受体(NMDAR)和AMPA受体(AMPAR)突触后介导的。生理数据表明,RGC处的谷氨酸受体不仅在突触后表达,而且在突触周围或突触外膜区室表达。但是,尚未确定RGC突触中谷氨酸受体的精确解剖位置。尽管广泛采用了中央突触的谷氨酸受体的高分辨率定量分析,但是这种方法在视网膜中仅获得了有限的成功。我们开发了一种包埋后免疫金的方法来分析膜受体,从而有可能估计视网膜带状突触中这些受体的数量,密度和变异性。在这里,我们描述了所需的工具,试剂和实际步骤:1)成功准备视网膜固定; 2)冷冻替代; 3)包埋后免疫金电子显微镜(EM)免疫细胞化学;以及4)谷氨酸受体的定量可视化在丝带突触。

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