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一种用于培养细胞内抗原的电子显微镜免疫细胞化学定位的新型初级固定剂的研发。

Development of a new primary fixative for electron microscopic immunocytochemical localization of intracellular antigens in cultured cells.

作者信息

Willingham M C, Yamada S S

出版信息

J Histochem Cytochem. 1979 May;27(5):947-60. doi: 10.1177/27.5.90071.

Abstract

We have developed a new primary fixative that permits the localization of intracellular antigens with well preserved ultrastructural morphology. This primary fixation method employs a mixture of a water soluble carbodiimide with glutaraldehyde, and preserves morphology, yet produces a permeable cytosol matrix so that antibodies can gain access to fixed proteins. Cultured cells were primarily fixed, treated with detergent to permeabilize their membranes, reacted with peroxidase labeled antibodies, secondarily fixed, and embedded in situ. The variations in morphology and accessibility of intracellular antigens were evaluated for a variety of fixatives. Concanavalin A and alpha 2 macroglobulin were chosen as examples of intracellular protein antigens to evaluate these fixation methods. Both of the proteins were localized in intracellular vesicles.

摘要

我们研发了一种新型的初级固定剂,它能够在超微结构形态得到良好保存的情况下对细胞内抗原进行定位。这种初级固定方法采用了水溶性碳二亚胺与戊二醛的混合物,既能保存形态,又能产生可渗透的细胞质基质,使抗体能够接触到固定的蛋白质。培养的细胞首先进行固定,用去污剂处理以使其膜通透,与过氧化物酶标记的抗体反应,然后进行二次固定,并原位包埋。针对多种固定剂,评估了细胞内抗原在形态和可及性方面的差异。选择伴刀豆球蛋白A和α2巨球蛋白作为细胞内蛋白质抗原的实例来评估这些固定方法。这两种蛋白质都定位在细胞内小泡中。

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