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在为超微结构免疫细胞化学进行最佳固定的组织切片中检测浆细胞免疫球蛋白。

Detection of plasma cell immunoglobulins in tissue sections optimally fixed for ultrastructural immunocytochemistry.

作者信息

Gonatas N K, Gonatas J O, Stieber A, Ternynck T, Avrameas S

出版信息

J Histochem Cytochem. 1987 Feb;35(2):189-96. doi: 10.1177/35.2.3098833.

Abstract

We describe the ultrastructural localization of plasma cell immunoglobulins in vibratome sections of popliteal lymph nodes. Fixation with glutaraldehyde-paraformaldehyde gave better tissue and antigen preservation than paraformaldehyde or periodic acid lysine-paraformaldehyde; biotinylated Fab fragments of sheep anti-mouse IgG-streptavidin-biotinylated horseradish peroxidase (HRP) or Fab-HRP conjugates gave similar results. With both immunoreagents, excellent tissue preservation and antigen detection was observed in the first layer of cells sectioned with the vibratome. Conjugates of anti-mouse IgG with HRP did not show any staining. Peroxidase stain was observed in the nuclear envelope, cisternae of the rough endoplasmic reticulum, and the Golgi apparatus complex. In the Golgi apparatus, staining was seen consistently in cisternae of the cis face and in adjacent vesicles; the trans cisternae showed weak or no stain, and adjacent vesicles, "coated" vesicles, and granules were not stained. This study shows that high quality of tissue preservation and antigen detection, by both light and ultrastructural immunocytochemistry, is feasible in tissue fixed with glutaraldehyde-paraformaldehyde followed by vibratome sectioning and immunostaining with Fab-biotin-streptavidin-biotin-HRP, or Fab-HRP.

摘要

我们描述了在腘淋巴结振动切片中浆细胞免疫球蛋白的超微结构定位。与多聚甲醛或高碘酸赖氨酸 - 多聚甲醛相比,用戊二醛 - 多聚甲醛固定能更好地保存组织和抗原;羊抗小鼠IgG - 链霉亲和素 - 生物素化辣根过氧化物酶(HRP)的生物素化Fab片段或Fab - HRP缀合物给出了相似的结果。使用这两种免疫试剂,在用振动切片机切片的第一层细胞中观察到了出色的组织保存和抗原检测。抗小鼠IgG与HRP的缀合物未显示任何染色。在核膜、粗面内质网的池和高尔基体复合体中观察到过氧化物酶染色。在高尔基体中,始终在顺面的池和相邻的小泡中看到染色;反面的池显示弱染色或无染色,相邻的小泡、“有被”小泡和颗粒未染色。这项研究表明,通过光镜和超微结构免疫细胞化学,在用戊二醛 - 多聚甲醛固定、随后进行振动切片并用Fab - 生物素 - 链霉亲和素 - 生物素 - HRP或Fab - HRP进行免疫染色的组织中,高质量的组织保存和抗原检测是可行的。

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