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Imaging Neurons within Thick Brain Sections Using the Golgi-Cox Method

机译:使用高尔基-柯克斯方法对脑厚部内的神经元进行成像

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摘要

The Golgi-Cox method of neuron staining has been employed for more than two hundred years to advance our understanding of neuron morphology within histological brain samples. While it is preferable from a practical perspective to prepare brain sections at the greatest thickness possible, in order to increase the probability of identifying stained neurons that are fully contained within single sections, this approach is limited from a technical perspective by the working distance of high-magnification microscope objectives. We report here a protocol to stain neurons using the Golgi-Cox method in mouse brain sections that are cut at 500 μm thickness, and to visualize neurons throughout the depth of these sections using an upright microscope fitted with a high-resolution 30X 1.05 N.A. silicone oil-immersion objective that has an 800 μm working distance. We also report two useful variants of this protocol that may be employed to counterstain the surface of mounted brain sections with the cresyl violet Nissl stain, or to freeze whole brains for long-term storage prior to sectioning and final processing. The main protocol and its two variants produce stained thick brain sections, throughout which full neuron dendritic trees and dendrite spines may be reliably visualized and quantified.
机译:神经元染色的高尔基-考克斯(Golgi-Cox)方法已经使用了200多年,以增进我们对组织学脑样本中神经元形态的理解。尽管从实用的角度出发,最好以尽可能最大的厚度准备大脑切片,但为了提高识别单个切片中完全包含的染色神经元的可能性,但从技术角度来看,这种方法的工作距离有限。放大显微镜物镜。我们在这里报告了一种协议,该协议使用高尔基-柯克斯方法在500微米厚的小鼠大脑切片中对神经元进行染色,并使用配备有高分辨率30X 1.05 NA硅酮的立式显微镜可视化这些切片的整个深度的神经元工作距离为800μm的油浸物镜。我们还报告了该协议的两个有用的变体,可用于使用甲酚紫Nissl染色剂对已安装的大脑切片的表面进行复染,或冻结整个大脑以在切片和最终加工之前长期保存。主要协议及其两个变体产生染色的厚脑节,整个神经元树突树和树突棘可以被可​​靠地可视化和量化。

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