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通过体外放射自显影对解冻装片的大鼠和人类前列腺组织切片中占据的雄激素受体进行定位和测量。

Localization and measurement of occupied androgen receptors in thaw-mounted rat and human prostate tissue sections by in vitro autoradiography.

作者信息

Brown T J, Sharma M, MacLusky N J

机构信息

Division of Reproductive Science, Toronto Hospital Research Institute, Ontario, Canada.

出版信息

Steroids. 1995 Feb;60(2):239-47. doi: 10.1016/0039-128x(94)00045-e.

DOI:10.1016/0039-128x(94)00045-e
PMID:7618192
Abstract

In this paper we present an in vitro exchange binding assay procedure for measurement of androgen receptors in slide-mounted tissue sections. This method allows quantitative autoradiographic determinations with an anatomical resolution approaching the cellular level. Tissue sections are incubated with the synthetic androgen [3H]R1881 in the presence of triamcinolone acetonide to suppress possible binding of the radioligand to the progestin receptor. Adjacent tissue sections are incubated with [3H]R1881 in the presence of excess unlabeled 5 alpha- dihydrotestosterone or R1881 to assess nonspecific binding. Following incubation, the tissue sections are washed to remove unbound radioligand and either scraped for immediate determination of androgen receptor binding or placed against emulsion-coated film for the production of an autoradiographic image. In validation experiments with rat prostate sections from castrated, gonad-intact, and androgen-supplemented animals, maximum levels of androgen binding were observed with incubation at 4 degrees C or 72 h. Markedly less binding was detected with shorter incubations or with incubations at even slightly elevated temperatures. Very little androgen receptor binding was detected in castrated animals whereas receptor levels in intact and androgen-supplemented animals were 79.3 fmol/mg and 143.6 fmol/mg protein, respectively, suggesting that the method is selective for occupied receptors. Saturation binding analysis revealed binding to a single class binding site with high affinity (kd = 1.475 +/- 0.12 nM). Autoradiographic images of androgen binding in the prostate reflected the findings with the scraped sections: essentially no specific binding was present in sections from castrated animals whereas much heavier labeling was present in sections from intact animals.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在本文中,我们介绍了一种用于测量载玻片上组织切片中雄激素受体的体外交换结合测定方法。该方法允许进行定量放射自显影测定,其解剖分辨率接近细胞水平。组织切片在曲安奈德存在的情况下与合成雄激素[³H]R1881一起孵育,以抑制放射性配体与孕激素受体的可能结合。相邻的组织切片在过量未标记的5α-双氢睾酮或R1881存在的情况下与[³H]R1881一起孵育,以评估非特异性结合。孵育后,将组织切片洗涤以去除未结合的放射性配体,然后刮下用于立即测定雄激素受体结合,或者放置在涂有乳剂的胶片上以产生放射自显影图像。在用去势、性腺完整和补充雄激素的动物的大鼠前列腺切片进行的验证实验中,在4℃孵育72小时时观察到雄激素结合的最大水平。较短的孵育时间或在甚至略微升高的温度下孵育时,检测到的结合明显较少。在去势动物中检测到的雄激素受体结合非常少,而完整和补充雄激素的动物中的受体水平分别为79.3 fmol/mg和143.6 fmol/mg蛋白质,这表明该方法对占据的受体具有选择性。饱和结合分析显示与具有高亲和力(kd = 1.475 +/- 0.12 nM)的单一类结合位点结合。前列腺中雄激素结合的放射自显影图像反映了刮下切片的结果:去势动物的切片中基本上没有特异性结合,而完整动物的切片中标记更重。(摘要截断于250字)

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