Preservation and immunogold localization of lipids by freeze-substitution and low temperature embedding.

Scanning microscopy. Supplement Pub Date : 1991-01-01
W Voorhout, I van Genderen, G van Meer, H Geuze
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Abstract

The success of post-embedding immunocytochemistry depends largely on the preparation methods. The requirements for structural preservation and immunocytochemistry are in some cases contradictory. This is especially the case in the study of lipid-rich structures and the localization of lipid components. Earlier work on freeze-substitution has shown that this method is very promising for the preservation of lipids and the immunocytochemical localization of lipids at the electron microscopical level. In this study we show that freeze-substitution in combination with low temperature embedding in Lowicryl HM20 has fulfilled this promise. Lamellar bodies in alveolar type II cells contain about 90% lipids and are very difficult to preserve in ultrathin cryosections. Lowicryl sections of freeze-substituted lung tissue shows excellent preservation of lamellar bodies in combination with immunogold localization of a hydrophobic surfactant protein. With an antibody against the Forssman glycolipid we demonstrate a highly reproducible intracellular localization of this glycolipid with high specificity and resolution. This method results in the retention of lipids and glycolipids and allows postembedding immunogold labeling.

冷冻取代和低温包埋法保存脂质及免疫金定位。
包埋后免疫细胞化学的成功在很大程度上取决于制备方法。结构保存和免疫细胞化学的要求在某些情况下是矛盾的。在研究富脂结构和脂质成分定位时尤其如此。早期关于冷冻取代的研究表明,这种方法在电子显微镜水平上对脂质的保存和脂质的免疫细胞化学定位非常有希望。在这项研究中,我们表明冷冻取代结合低温包埋在Lowicryl HM20中实现了这一希望。肺泡II型细胞的片层体含有约90%的脂质,很难在超薄冷冻中保存。冷冻替代肺组织的低丙基切片显示,结合疏水表面活性剂蛋白的免疫金定位,片层体得到了很好的保存。使用针对Forssman糖脂的抗体,我们证明了这种糖脂具有高特异性和高分辨率的高度可重复的细胞内定位。这种方法导致脂质和糖脂质的保留,并允许包埋后免疫金标记。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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