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下丘脑神经元的包埋前胶体金免疫染色:β-内啡肽免疫反应性胞体的光镜和电镜定位

Preembedding colloidal gold immunostaining of hypothalamic neurons: light and electron microscopic localization of beta-endorphin-immunoreactive perikarya.

作者信息

Lamberts R, Goldsmith P C

出版信息

J Histochem Cytochem. 1985 Jun;33(6):499-507. doi: 10.1177/33.6.2582027.

DOI:10.1177/33.6.2582027
PMID:2582027
Abstract

A preembedding immunogold staining (IGS) procedure was developed to identify beta-endorphin/adrenocorticotropic hormone immunoreactive neurons at the light and electron microscopic levels. Colchicine-treated rats were perfused with Nakane's periodate-lysine-paraformaldehyde fixative. Vibratome sections were incubated in primary antisera followed by goat anti-rabbit immunoglobulin G coupled to 16 nm colloidal gold, and, in some cases, rabbit immunoglobulin G coupled to gold. The appearance to pink to light red perikarya, corresponding to colloidal gold deposition at antigenic sites, was monitored under the light microscope. Positive cell bodies in the arcuate region sometimes extended lateral to the nucleus. Only proximal portions of neuronal processes were stained. At the ultrastructural level, colloidal gold labeled the periphery of 90-110 nm dense neurosecretory granules in the perikaryal cytoplasm and a few proximal axons. Clusters of gold particles, appearing free in the neuroplasm, actually labeled secretory granules in adjacent thin sections. Granules associated with the Golgi apparatus were not stained. Colloidal gold labeling of mature beta-endorphin granules, but not progranules, in rat hypothalamic neurons was confirmed using the peroxidase-antiperoxidase technique. The results correlate well with data on the intracellular processing of pro-opiomelanocortin in pituitary cells and prepropressophysin in the paraventricular nucleus. These data demonstrate the first application of the preembedding colloidal gold staining method for the identification of intracellular antigens within the central nervous system. The IGS method provides a definitive marker for single or double labeling of nervous tissue at both the light and electron microscopic levels.

摘要

我们开发了一种包埋前免疫金染色(IGS)程序,用于在光学和电子显微镜水平上识别β-内啡肽/促肾上腺皮质激素免疫反应性神经元。用秋水仙碱处理的大鼠用中根过碘酸盐-赖氨酸-多聚甲醛固定剂灌注。振动切片机切片在一抗中孵育,然后与结合了16nm胶体金的山羊抗兔免疫球蛋白G孵育,在某些情况下,还与结合了金的兔免疫球蛋白G孵育。在光学显微镜下监测对应于抗原位点胶体金沉积的粉红色至浅红色核周体的外观。弓状区域的阳性细胞体有时延伸到细胞核的外侧。仅神经元突起的近端部分被染色。在超微结构水平上,胶体金标记了核周细胞质中90-110nm致密神经分泌颗粒的周边以及一些近端轴突。在神经浆中看似游离的金颗粒簇,实际上标记了相邻薄切片中的分泌颗粒。与高尔基体相关的颗粒未被染色。使用过氧化物酶-抗过氧化物酶技术证实了大鼠下丘脑神经元中成熟β-内啡肽颗粒而非前颗粒的胶体金标记。这些结果与垂体细胞中阿片促黑激素原和室旁核中前促肾上腺皮质激素释放激素原的细胞内加工数据密切相关。这些数据证明了包埋前胶体金染色方法在中枢神经系统内细胞内抗原鉴定中的首次应用。IGS方法为神经组织在光学和电子显微镜水平上的单标记或双标记提供了一种明确的标记物。

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Preembedding colloidal gold immunostaining of hypothalamic neurons: light and electron microscopic localization of beta-endorphin-immunoreactive perikarya.下丘脑神经元的包埋前胶体金免疫染色:β-内啡肽免疫反应性胞体的光镜和电镜定位
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