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转基因表达的免疫组织化学分析。

Immunohistochemical analysis of transgene expression.

作者信息

Funkhouser J M

机构信息

Neuropeptide Laboratory, Institute of Molecular and Cell Biology, National University of Singapore, Republic of Singapore.

出版信息

Methods Mol Biol. 1993;18:395-405. doi: 10.1385/0-89603-245-0:395.

DOI:10.1385/0-89603-245-0:395
PMID:21390686
Abstract

Immunohistochemistry can be used to localize the peptide or protein product of the transgene, or to identify particular cell types within tissue sections by labeling a specific protein. There are many ways to do this. Today many involve a primary antibody to the protein of interest, and a secondary antibody plus a fluorescent or enzyme tag to visualize the reaction. The fluorescent tag is observed by viewing it through a microscope equipped with a light source of the correct wavelength to excite the molecules of the tag, which then emit light of a specific wavelength, visible through filters. Because the fluorescent material contains a limited number of molecules, the label is temporary and needs to be photographed to save the result obtained. The second protocol given here uses a fluorescent tag. In contrast, the enzymes alkaline phosphatase and horseradish peroxidase can be visualized with chromogens that create a permanent slide, which can be examined immediately in a simple bright-field microscope and reviewed later. Additionally, it allows a clear bright-field or Nomarski view of the tissue, together with the label. These approaches give a one-enzyme molecule for one antibody-antigen reaction. For proteins in low abundance, the reaction may be enhanced by Sternberger's peroxidase antiperoxidase (PAP) method, which attaches a three-enzyme complex to the secondary antibody. Alternatively, the enhancement is accomplished by using a biotin-labeled secondary antibody that binds a streptavidin molecule complexed to enzyme molecules. The latter approach is the first method described here. It has yielded good results in a variety of tissues, and, with the correct dilution of the antibodies and streptavidin complex, results in a clear signal.

摘要

免疫组织化学可用于定位转基因的肽或蛋白质产物,或通过标记特定蛋白质来识别组织切片中的特定细胞类型。有多种方法可以做到这一点。如今,许多方法涉及针对感兴趣蛋白质的一抗,以及带有荧光或酶标记的二抗以可视化反应。通过配备有正确波长光源的显微镜观察荧光标记,该光源可激发标记分子,然后标记分子会发出特定波长的光,通过滤光片可见。由于荧光物质包含的分子数量有限,标记是暂时的,需要拍照以保存获得的结果。此处给出的第二个方案使用荧光标记。相比之下,碱性磷酸酶和辣根过氧化物酶可以用发色剂可视化,从而制作出永久玻片,可在简单的明场显微镜下立即检查并在以后复查。此外,它还能提供组织以及标记的清晰明场或诺马斯基视图。这些方法在一次抗体 - 抗原反应中产生一个酶分子。对于低丰度蛋白质,反应可通过斯特恩伯格过氧化物酶抗过氧化物酶(PAP)方法增强,该方法将一个三酶复合物连接到二抗上。或者,通过使用与结合了酶分子的链霉亲和素分子复合的生物素标记二抗来实现增强。后一种方法是此处描述的第一种方法。它在各种组织中都取得了良好的效果,并且通过正确稀释抗体和链霉亲和素复合物,可产生清晰的信号。

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