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用于在电压钳制条件下检查哺乳动物神经肌肉传递的耳长提肌制备

Levator Auris Longus Preparation for Examination of Mammalian Neuromuscular Transmission Under Voltage Clamp Conditions.

作者信息

Burke Steven R A, Reed Eric J, Romer Shannon H, Voss Andrew A

机构信息

Department of Biological Sciences, Wright State University.

Department of Biological Sciences, Wright State University;

出版信息

J Vis Exp. 2018 May 5(135):57482. doi: 10.3791/57482.

Abstract

This protocol describes a technique to record synaptic transmission from the neuromuscular junction under current-clamp and voltage-clamp conditions. An ex vivo preparation of the levator auris longus (LAL) is used because it is a thin muscle that provides easy visualization of the neuromuscular junction for microelectrode impalement at the motor endplate. This method allows for the recording of spontaneous miniature endplate potentials and currents (mEPPs and mEPCs), nerve-evoked endplate potentials and currents (EPPs and EPCs), as well as the membrane properties of the motor endplate. Results obtained from this method include the quantal content (QC), number of vesicle release sites (n), probability of vesicle release (prel), synaptic facilitation and depression, as well as the muscle membrane time constant (τm) and input resistance. Application of this technique to mouse models of human disease can highlight key pathologies in disease states and help identify novel treatment strategies. By fully voltage-clamping a single synapse, this method provides one of the most detailed analyses of synaptic transmission currently available.

摘要

本方案描述了一种在电流钳制和电压钳制条件下记录神经肌肉接头处突触传递的技术。使用离体的耳长提肌(LAL)标本,因为它是一块薄肌肉,便于在运动终板处对神经肌肉接头进行可视化,以便微电极刺入。该方法允许记录自发的微小终板电位和电流(mEPPs和mEPCs)、神经诱发的终板电位和电流(EPPs和EPCs)以及运动终板的膜特性。从该方法获得的结果包括量子含量(QC)、囊泡释放位点数量(n)、囊泡释放概率(prel)、突触易化和抑制,以及肌肉膜时间常数(τm)和输入电阻。将该技术应用于人类疾病的小鼠模型可以突出疾病状态下的关键病理,并有助于确定新的治疗策略。通过对单个突触进行完全电压钳制,该方法提供了目前可用的对突触传递最详细的分析之一。

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