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大鼠原生脑的高压冷冻和冷冻置换:用于髓鞘糖脂的保存及免疫电子显微镜定位的适用性

High-pressure freezing and freeze-substitution of native rat brain: suitability for preservation and immunoelectron microscopic localization of myelin glycolipids.

作者信息

Kirschning E, Rutter G, Hohenberg H

机构信息

Heinrich-Pette-Institute for Experimental Virology and Immunology at the University of Hamburg, Germany.

出版信息

J Neurosci Res. 1998 Aug 15;53(4):465-74. doi: 10.1002/(SICI)1097-4547(19980815)53:4<465::AID-JNR8>3.0.CO;2-4.

Abstract

Galactocerebroside (GalC) and sulfatide are major constituent lipids in vertebrate myelin. Their precise immunolocalization in electron microscopy so far has been hampered by the fact that lipids are not immobilized by chemical fixation and thus get extracted during dehydration with organic solvents. Here, we examined the suitability of cryotechniques for the preservation and immunohistochemical localization of myelin glycolipids in rat brain at the ultrastructural level. Native cerebral cortex tissue, obtained by fine-needle biopsy, was cryoimmobilized by high-pressure freezing and dehydrated by freeze-substitution before embedding in Epon. This procedure resulted in an excellent preservation of brain ultrastructure. Concomitantly, immunogold labeling of ultrathin sections with the well-defined monoclonal antibodies (mAbs) O1, O4, and R-mAb, which were shown to react with GalC and/or sulfatide and some structurally related glycolipids, revealed a good conservation of relevant epitopes. These data suggest that in adult rat cerebral cortex, the most relevant antigens recognized by R-mAb, O1, and O4, namely GalC and sulfatide, are exclusively expressed in myelin structures. Because these mAbs are common markers for the identification of developing oligodendrocytes, this "postembedding glycolipid-labeling technique" holds great potential for studying oligodendroglial differentiation in normal and pathological conditions at the ultrastructural level.

摘要

半乳糖脑苷脂(GalC)和硫脂是脊椎动物髓鞘中的主要脂质成分。迄今为止,脂质在电子显微镜下的精确免疫定位受到阻碍,因为脂质不能通过化学固定固定下来,因此在有机溶剂脱水过程中会被提取出来。在此,我们在超微结构水平上研究了低温技术对大鼠脑髓鞘糖脂的保存和免疫组织化学定位的适用性。通过细针活检获得的天然大脑皮质组织,通过高压冷冻进行冷冻固定,并在嵌入环氧树脂之前通过冷冻置换进行脱水。该程序导致脑超微结构得到了极好的保存。同时,用已证明与GalC和/或硫脂以及一些结构相关的糖脂发生反应的明确单克隆抗体(mAb)O1、O4和R-mAb对超薄切片进行免疫金标记,显示相关表位得到了良好的保存。这些数据表明,在成年大鼠大脑皮质中,R-mAb、O1和O4识别的最相关抗原,即GalC和硫脂,仅在髓鞘结构中表达。由于这些单克隆抗体是鉴定发育中的少突胶质细胞的常用标志物,这种“包埋后糖脂标记技术”在超微结构水平研究正常和病理条件下少突胶质细胞分化方面具有巨大潜力。

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