Electron Microscopic Methods for Determining Changes in the Density of Synaptic Input to Neurons in the Aging Brain

Witkin Joan W.
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引用次数: 1

Abstract

Changes in the synaptic input to aging neurons can best be evaluated using electron microscopy (EM). Immunocytochemistry is used to identify neuronal populations and to distinguish the chemical identity of their synaptic input, using a double-label protocol (e.g., diaminobenzidine for the sites of the first antigen/antibody complexes and tetramethylbenzidine for the second). In preparing tissue for EM examination, neurons are sectioned in the plane of the nucleus at 70 nm and sections collected on slot hole grids. Photographic montages of neurons are made at a minimum of 3 depths of section, with about 1 μm intervening. The original micrographs are taken at 10,000× and printed at 25,000×. Morphometric analyses are performed using the Bloquant program (R&M Biometrics) and an IBM computer. The perikaryal membrane is outlined on an X-Y digitizing pad, and regions along which there is synaptic modification are measured. These synaptic regions are expressed as a percentage of the perikaryal membrane measured. Data are tested using a non-parametric statistic (Mann-Whitney U, P < 0.05). In some cases, the entire neuronal soma is serially sectioned in order to determine whether synapses are randomly distributed over the neuronal surface.

测定衰老大脑神经元突触输入密度变化的电镜方法
衰老神经元突触输入的变化可以最好地使用电子显微镜(EM)来评估。免疫细胞化学用于识别神经元群体,并使用双重标记方案(例如,第一个抗原/抗体复合物的位点为二氨基联苯胺,第二个位点为四甲基联苯胺)来区分其突触输入的化学特性。在准备用于EM检查的组织时,在70nm的细胞核平面中对神经元进行切片,并将切片收集在槽孔网格上。神经元的摄影蒙太奇是在至少3个深度的剖面上制作的,中间大约有1μm。原始显微照片是以10000×拍摄的,并以25000×打印。使用Bloquant程序(R&;M Biometrics)和IBM计算机进行形态计量分析。在X-Y数字化垫上勾勒出卡周膜的轮廓,并测量突触修饰的区域。这些突触区域以所测量的卡周膜的百分比表示。使用非参数统计(Mann-Whitney U,P<;0.05)测试数据。在某些情况下,为了确定突触是否随机分布在神经元表面,对整个神经元胞体进行连续切片。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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