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用于透射电子显微镜(TEM)的伦敦树脂(LR)白色切片的免疫金染色。

Immunogold Staining of London Resin (LR) White Sections for Transmission Electron Microscopy (TEM).

作者信息

Skepper Jeremy N, Powell Janet M

出版信息

CSH Protoc. 2008 Jun 1;2008:pdb.prot5016. doi: 10.1101/pdb.prot5016.

Abstract

INTRODUCTIONIn post-embedding methods of immunogold staining, the cells or tissues are fixed chemically or cryoimmobilized, dehydrated, and embedded in epoxy or acrylic resins. Thin sections (50-70 nm in thickness) are cut using an ultramicrotome with a diamond knife, using a water bath to collect the sections as they slide off the knife. The sections are stretched with solvent vapor or a heat source and collected onto either bare or plastic-coated nickel grids. The sections are then stained immunochemically with primary antibodies raised against antigens exposed on the surface of the sections. The primary antibodies are visualized by staining immunochemically with secondary antibodies raised against the species and isotype of the primary antibodies, conjugated to colloidal gold particles. The immunochemically stained sections are then contrast stained with salts of uranium (uranyl acetate) and lead (lead citrate) to reveal the ultrastructure of the cells, and are finally viewed by transmission electron microscopy (TEM). LR White was introduced as a low-toxicity alternative to epoxy resins, which frequently contained carcinogens. Unlike the simplest acrylic resins, in which monomers are polymerized to form long chains, the LR resins contain aromatic cross-linkers to improve the stability of the sections under the electron beam. LR White and Gold both have very low viscosity and readily penetrate, even into dense tissue. In this protocol, aldehyde-fixed tissue is dehydrated in ethanol, impregnated in LR White resin and polymerized under vacuum or in a nitrogen atmosphere before sectioning and immunogold staining.

摘要

引言

在免疫金染色的包埋后方法中,细胞或组织通过化学固定或冷冻固定、脱水,然后包埋在环氧树脂或丙烯酸树脂中。使用配备金刚石刀的超薄切片机切出厚度为50 - 70纳米的薄片,切片从刀上滑落时,利用水浴收集切片。切片用溶剂蒸汽或热源拉伸,然后收集到裸露的或涂有塑料的镍网上。接着用针对切片表面暴露抗原产生的一抗进行免疫化学染色。通过用针对一抗的物种和同种型产生的二抗进行免疫化学染色来使一抗可视化,二抗与胶体金颗粒偶联。然后对免疫化学染色的切片用铀盐(醋酸双氧铀)和铅盐(柠檬酸铅)进行对比染色,以揭示细胞的超微结构,最后通过透射电子显微镜(TEM)观察。LR White作为环氧树脂的低毒性替代品被引入,环氧树脂通常含有致癌物。与最简单的丙烯酸树脂不同,在最简单的丙烯酸树脂中单体聚合形成长链,而LR树脂含有芳香族交联剂以提高切片在电子束下的稳定性。LR White和Gold的粘度都非常低,即使是致密组织也能很容易地渗透进去。在本方案中,醛固定的组织在乙醇中脱水,用LR White树脂浸渍,并在真空或氮气气氛下聚合,然后进行切片和免疫金染色。

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