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镜像技术在神经化学鉴定的γ-氨基丁酸能树突三维电子显微镜检查中的应用。

Application of the Mirror Technique for Three-Dimensional Electron Microscopy of Neurochemically Identified GABA-ergic Dendrites.

作者信息

Talapka Petra, Kocsis Zsolt, Marsi Lívia Diána, Szarvas Vera Etelka, Kisvárday Zoltán F

机构信息

MTA-DE Neuroscience Research Group, University of Debrecen, Debrecen, Hungary.

Department of Anatomy, Histology and Embryology, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.

出版信息

Front Neuroanat. 2021 Apr 20;15:652422. doi: 10.3389/fnana.2021.652422. eCollection 2021.

Abstract

In the nervous system synaptic input arrives chiefly on dendrites and their type and distribution have been assumed pivotal in signal integration. We have developed an immunohistochemistry (IH)-correlated electron microscopy (EM) method - the "mirror" technique - by which synaptic input to entire dendrites of neurochemically identified interneurons (INs) can be mapped due preserving high-fidelity tissue ultrastructure. Hence, this approach allows quantitative assessment of morphometric parameters of synaptic inputs along the whole length of dendrites originating from the parent soma. The method exploits the fact that adjoining sections have truncated or cut cell bodies which appear on the common surfaces in a mirror fashion. In one of the sections the histochemical marker of the GABAergic subtype, calbindin was revealed in cell bodies whereas in the other section the remaining part of the very same cell bodies were subjected to serial section EM to trace and reconstruct the synaptology of entire dendrites. Here, we provide exemplary data on the synaptic coverage of two dendrites belonging to the same calbindin-D immunopositive IN and determine the spatial distribution of asymmetric and symmetric synapses, surface area and volume of the presynaptic boutons, morphometric parameters of synaptic vesicles, and area extent of the active zones.

摘要

在神经系统中,突触输入主要到达树突,并且其类型和分布被认为在信号整合中起关键作用。我们开发了一种免疫组织化学(IH)相关的电子显微镜(EM)方法——“镜像”技术,通过该技术可以绘制神经化学鉴定的中间神经元(INs)整个树突的突触输入,同时保留高保真的组织超微结构。因此,这种方法允许对源自母细胞体的树突全长上的突触输入的形态测量参数进行定量评估。该方法利用了相邻切片具有截断或切割的细胞体这一事实,这些细胞体以镜像方式出现在共同表面上。在其中一个切片中,GABA能亚型的组织化学标记物钙结合蛋白在细胞体中显示出来,而在另一个切片中,同一细胞体的其余部分进行连续切片EM,以追踪和重建整个树突的突触学。在这里,我们提供了属于同一钙结合蛋白-D免疫阳性IN的两个树突的突触覆盖的示例性数据,并确定了不对称和对称突触的空间分布、突触前终扣的表面积和体积、突触小泡的形态测量参数以及活性区的面积范围。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d9f7/8093522/b83853e7ad57/fnana-15-652422-g001.jpg

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