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用生物素化抗体进行预包埋标记,随后对薄切片上暴露的生物素基团进行可视化。

Preembedding labeling with biotinylated antibodies and subsequent visualization of the biotin groups exposed on thin sections.

作者信息

Nir I, Schneider B G, Papermaster D S

出版信息

J Histochem Cytochem. 1984 Jun;32(6):643-8. doi: 10.1177/32.6.6233358.

Abstract

The feasibility of labeling cell membranes with biotinylated ligands and detecting the biotin groups on thin sections was investigated. Fixed retinal tissue was incubated with biotinyl- antiopsin . Half of the biotinyl-antibody labeled retinal tissue was incubated with avidin-ferritin (AvF) and embedded in Epon (preembedding reaction). The second half was embedded in glutaraldehyde cross-linked bovine serum albumin (BSA). Thin sections of this preparation were incubated with AvF to detect biotinyl-antibodies exposed by the sectioning (postembedding reaction). Biotin groups on the thin section surface could be readily visualized with AvF. Stereoscopic images demonstrated that the ferritin particles were localized only on the exposed surface of the thin section. The labeling was highly specific, with a very low background. Quantitative analysis was employed in order to determine the optimal reaction conditions for maximizing the labeling density with minimizing nonspecific binding. The possibility of using biotinylated molecules in the study of dynamic cellular events and for the subsequent intracellular localization of biotin on thin sections is suggested.

摘要

研究了用生物素化配体标记细胞膜并在薄切片上检测生物素基团的可行性。将固定的视网膜组织与生物素化抗视蛋白一起孵育。一半生物素化抗体标记的视网膜组织与抗生物素蛋白-铁蛋白(AvF)一起孵育并包埋在环氧树脂中(包埋前反应)。另一半包埋在戊二醛交联的牛血清白蛋白(BSA)中。该制剂的薄切片与AvF一起孵育,以检测切片暴露的生物素化抗体(包埋后反应)。薄切片表面的生物素基团可用AvF轻松可视化。立体图像显示铁蛋白颗粒仅定位在薄切片的暴露表面。标记具有高度特异性,背景非常低。采用定量分析以确定最佳反应条件,以在最小化非特异性结合的同时最大化标记密度。提出了在动态细胞事件研究中使用生物素化分子以及随后在薄切片上进行生物素细胞内定位的可能性。

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