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成像大鼠原代海马神经元树突棘使用结构照明显微镜

JoVE Journal
Neuroscienze

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JoVE Journal Neuroscienze

Imaging Dendritic Spines of Rat Primary Hippocampal Neurons using Structured Illumination Microscopy

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成像大鼠原代海马神经元树突棘使用结构照明显微镜

DOI:

10.3791/51276-v

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14:11 min

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May 04, 2014

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Marijn Schouten*¹, Giulia M. R. De Luca*², Diana K. Alatriste González, Babette E. de Jong, Wendy Timmermans, Hui Xiong, Harm Krugers, Erik M. M. Manders, Carlos P. Fitzsimons

¹Center for Neuroscience, Swammerdam Institute for Life Sciences,University of Amsterdam, ²Van Leeuwenhoek Centre for Advanced Microscopy, Section Molecular Cytology, Swammerdam Institute for Life Sciences,University of Amsterdam

Capitoli

00:05Titolo
02:05Coverslip Preparation
02:48Dissection of the Hippocampi
03:58Cell Dissociation and Plating
05:35Rat Hippocampal Primary Neuron Transfection using Lipofectamine
07:23Immunostaining Hippocampal Primary Neurons
08:54Dendritic Spine Imaging using Structure Illumination Microscopy
12:12Results: Dendrites and Dendritic Spines Imaged with SIM and Confocal Microscopy
13:22Conclusion

Summary

Traduzione automatica

本文介绍了使用结构照明显微镜（SIM卡） 在体外海马神经元的工作协议，以形象的树突棘。使用SIM卡超高分辨率显微镜提供的图像分辨率显著超越在所有三个空间维度的光的衍射极限，允许单个树突棘与改进的细节的影像。

Tags

Dendritic Spines Rat Primary Hippocampal Neurons Structured Illumination Microscopy (SIM)Super-resolution Microscopy Neuronal Connectivity Synaptic Plasticity Neuron Culture Fluorescent Protein 3D Reconstruction

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