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多聚甲醛固定切片中双层免疫组织化学染色问题的研究

An investigation of the problem of two-layered immunohistochemical staining in paraformaldehyde fixed sections.

作者信息

Torres Eduardo M, Meldrum Alicia, Kirik Deniz, Dunnett Stephen B

机构信息

Cardiff University, School of Biosciences, Museum Avenue, Cardiff CF10 3US, United Kingdom.

出版信息

J Neurosci Methods. 2006 Nov 15;158(1):64-74. doi: 10.1016/j.jneumeth.2006.05.016. Epub 2006 Jun 23.

Abstract

In sections of paraformaldehyde fixed brain tissue, stained using immunohistochemical methods, the distribution of staining within the sections is not uniform. Whilst stained cells are seen at the top and bottom surfaces, the central thicknesses of the sections contain little or no immunoreactivity. This presents a major problem for quantification, as each section contains a population of cells that is not visualized by the staining method. Following extensive investigation of this phenomenon, we report that the failure of full thickness, immunohistochemical staining is not a failure of the immunohistochemical methodology per se, nor is it related directly to the thickness of the sections used. Rather, the problem lies in the chemistry of the tissue itself, and originates during fixation of the tissues using paraformaldehyde-based perfusion methods, which render the cell membranes impermeable to one or more components of the staining protocol. We show that this impermeability is affected by addition of membrane-disrupting agents to the fixative, and by a reduction of exposure to paraformaldehyde during fixation. The present investigation contributes to the development of new fixation protocols, optimised for use in both immunohistochemical methods and morphometric analyses.

摘要

在使用免疫组织化学方法染色的多聚甲醛固定脑组织切片中,切片内的染色分布并不均匀。虽然在切片的顶面和底面可见染色细胞,但切片的中心厚度区域几乎没有或没有免疫反应性。这给定量分析带来了一个主要问题,因为每个切片都包含一群无法通过染色方法观察到的细胞。在对这一现象进行广泛研究之后,我们报告全层免疫组织化学染色失败并非免疫组织化学方法本身的失败,也与所用切片的厚度没有直接关系。相反,问题在于组织本身的化学性质,并且源于使用基于多聚甲醛的灌注方法固定组织的过程中,这使得细胞膜对染色方案中的一种或多种成分不可渗透。我们表明,这种不可渗透性受到向固定剂中添加膜破坏剂以及在固定过程中减少多聚甲醛暴露时间的影响。本研究有助于开发新的固定方案,这些方案针对免疫组织化学方法和形态计量分析进行了优化。

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