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寻常型天疱疮表皮中体内结合免疫球蛋白的免疫化学定位。用于光学显微镜和电子显微镜的过氧化物酶-抗过氧化物酶多步技术的应用。

Immunochemical localization of in vivo bound immunoglobulins in pemphigus vulgaris epidermis. Employment of a peroxidase-antiperoxidase multistep technique for light and electron microscopy.

作者信息

Hönigsmann H, Holubar K, Wolff K, Beutner E H

出版信息

Arch Dermatol Res (1975). 1975 Dec 10;254(2):113-20. doi: 10.1007/BF00586886.

Abstract

A multi-step immunocytochemical method utilizing horseradish peroxidase (HRP) as an immunological marker was employed to demonstrate, at the ultrastructural level, IgG antiepithelial autoantibodies bound in vivo to pemphigus epidermis, and circulating IgG antibodies, using monkey oesophagus as substrate. To demonstrate IgG the following antisera were employed in sequential steps: Goat antihuman IgG; rabbit antigoat IgG; goat-anti-HRP-serum. After incubating with the final antigen, HRP, the latter was visualized with a cytochemical method. Results paralleled those obtained by immunofluorescence, the antiepithelial antibody being demonstrated at the sites of the intercellular spaces of the epidermis. Electron microscopic cytochemistry showed IgG in the surface coat of epidermal cells and in the intercellular space, both in the desmosomal and the interdesmosomal areas. These results confirm the results of a previous study but the localization of the antibody is more exact than that obtained with HRP-conjugates. The present method is more versatile and specific than HRP methods that utilize HRP-conjugated antibodies.

摘要

采用一种以辣根过氧化物酶(HRP)作为免疫标记物的多步免疫细胞化学方法,以猴食管为底物,在超微结构水平上证实天疱疮表皮中体内结合的IgG抗上皮自身抗体以及循环IgG抗体。为了证实IgG,按顺序步骤使用了以下抗血清:山羊抗人IgG;兔抗山羊IgG;山羊抗HRP血清。与最终抗原HRP孵育后,用细胞化学方法使后者显色。结果与免疫荧光法所得结果相似,抗上皮抗体在表皮细胞间间隙部位被证实。电子显微镜细胞化学显示,在桥粒和桥粒间区域的表皮细胞表面被膜和细胞间间隙中均有IgG。这些结果证实了先前一项研究的结果,但抗体的定位比使用HRP偶联物所获得的定位更为精确。本方法比利用HRP偶联抗体的HRP方法更具通用性和特异性。

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