首页> 美国卫生研究院文献>Journal of Visualized Experiments : JoVE >Preparation of Primary Neurons for Visualizing Neurites in a Frozen-hydrated State Using Cryo-Electron Tomography
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Preparation of Primary Neurons for Visualizing Neurites in a Frozen-hydrated State Using Cryo-Electron Tomography

机译:使用冷冻电子断层扫描技术在冷冻水合状态下可视化神经突的初级神经元的制备

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摘要

Neurites, both dendrites and axons, are neuronal cellular processes that enable the conduction of electrical impulses between neurons. Defining the structure of neurites is critical to understanding how these processes move materials and signals that support synaptic communication. Electron microscopy (EM) has been traditionally used to assess the ultrastructural features within neurites; however, the exposure to organic solvent during dehydration and resin embedding can distort structures. An important unmet goal is the formulation of procedures that allow for structural evaluations not impacted by such artifacts. Here, we have established a detailed and reproducible protocol for growing and flash-freezing whole neurites of different primary neurons on electron microscopy grids followed by their examination with cryo-electron tomography (cryo-ET). This technique allows for 3-D visualization of frozen, hydrated neurites at nanometer resolution, facilitating assessment of their morphological differences. Our protocol yields an unprecedented view of dorsal root ganglion (DRG) neurites, and a visualization of hippocampal neurites in their near-native state. As such, these methods create a foundation for future studies on neurites of both normal neurons and those impacted by neurological disorders.
机译:神经突,包括树突和轴突,都是神经元细胞过程,能够在神经元之间传导电脉冲。定义神经突的结构对于理解这些过程如何移动支持突触通讯的物质和信号至关重要。传统上,电子显微镜(EM)用于评估神经突内的超微结构特征。但是,在脱水和树脂包埋过程中暴露于有机溶剂会使结构变形。一个未实现的重要目标是制定程序,以使结构评估不受此类工件的影响。在这里,我们建立了详细且可重现的协议,用于在电子显微镜栅格上生长和快速冻结不同初级神经元的整个神经突,然后用低温电子断层扫描(cryo-ET)对其进行检查。这项技术允许以纳米级分辨率对冷冻的水合神经突进行3D可视化,从而有助于评估它们的形态差异。我们的协议产生了背根神经节(DRG)神经突的前所未有的视图,并以近乎自然的状态可视化了海马神经突。这样,这些方法为将来对正常神经元和受神经系统疾病影响的神经元的神经突的研究奠定了基础。

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