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从体内功能特征化的神经元中获得高产的体外记录。

High-yield in vitro recordings from neurons functionally characterized in vivo.

机构信息

Max Planck Institute of Neurobiology, München-Martinsried, Germany.

出版信息

Nat Protoc. 2018 Jun;13(6):1275-1293. doi: 10.1038/nprot.2018.026. Epub 2018 May 10.

Abstract

In vivo two-photon calcium imaging provides detailed information about the activity and response properties of individual neurons. However, in vitro methods are often required to study the underlying neuronal connectivity and physiology at the cellular and synaptic levels at high resolution. This protocol provides a fast and reliable workflow for combining the two approaches by characterizing the response properties of individual neurons in mice in vivo using genetically encoded calcium indicators (GECIs), followed by retrieval of the same neurons in brain slices for further analysis in vitro (e.g., circuit mapping). In this approach, a reference frame is provided by fluorescent-bead tracks and sparsely transduced neurons expressing a structural marker in order to re-identify the same neurons. The use of GECIs provides a substantial advancement over previous approaches by allowing for repeated in vivo imaging. This opens the possibility of directly correlating experience-dependent changes in neuronal activity and feature selectivity with changes in neuronal connectivity and physiology. This protocol requires expertise both in in vivo two-photon calcium imaging and in vitro electrophysiology. It takes 3 weeks or more to complete, depending on the time allotted for repeated in vivo imaging of neuronal activity.

摘要

在体双光子钙成像提供了关于单个神经元活动和反应特性的详细信息。然而,为了在细胞和突触水平上以高分辨率研究潜在的神经元连接和生理学,通常需要体外方法。本方案提供了一种快速可靠的工作流程,通过使用遗传编码钙指示剂(GECIs)对体内的单个神经元的反应特性进行特征描述,然后在脑片中取回相同的神经元进行进一步的体外分析(例如,回路映射),从而将这两种方法结合起来。在这种方法中,通过荧光珠轨迹和稀疏转导表达结构标记的神经元提供参考框架,以便重新识别相同的神经元。与以前的方法相比,GECIs 的使用通过允许重复的在体成像提供了实质性的进展。这使得直接将神经元活动和特征选择性的经验依赖性变化与神经元连接和生理学的变化相关联成为可能。该方案既需要在体双光子钙成像方面的专业知识,也需要在体外电生理学方面的专业知识。完成它需要 3 周或更长时间,具体取决于为重复进行的神经元活动的在体成像分配的时间。

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