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体内翻译后修饰蛋白质的高特异性抗体的产生和纯化。

Generation and purification of highly specific antibodies for detecting post-translationally modified proteins in vivo.

机构信息

Department of Genetics, The University of Texas M.D. Anderson Cancer Center, Houston, Texas, USA.

Department of Genetics, Washington University in St. Louis, St. Louis, Missouri, USA.

出版信息

Nat Protoc. 2014 Feb;9(2):375-95. doi: 10.1038/nprot.2014.017. Epub 2014 Jan 23.

Abstract

Post-translational modifications alter protein structure, affecting activity, stability, localization and/or binding partners. Antibodies that specifically recognize post-translationally modified proteins have a number of uses including immunocytochemistry and immunoprecipitation of the modified protein to purify protein-protein and protein-nucleic acid complexes. However, antibodies directed at modified sites on individual proteins are often nonspecific. Here we describe a protocol to purify polyclonal antibodies that specifically detect the modified protein of interest. The approach uses iterative rounds of subtraction and affinity purification, using stringent washes to remove antibodies that recognize the unmodified protein and low sequence complexity epitopes containing the modified amino acid. Dot blot and western blot assays are used to assess antibody preparation specificity. The approach is designed to overcome the common occurrence that a single round of subtraction and affinity purification is not sufficient to obtain a modified protein-specific antibody preparation. One full round of antibody purification and specificity testing takes 6 d of discontinuous time.

摘要

翻译后修饰改变蛋白质结构,影响其活性、稳定性、定位和/或结合伙伴。专门识别翻译后修饰蛋白的抗体有多种用途,包括免疫细胞化学和翻译后修饰蛋白的免疫沉淀,以纯化蛋白-蛋白和蛋白-核酸复合物。然而,针对单个蛋白上修饰位点的抗体通常是非特异性的。本文描述了一种纯化特异性识别感兴趣的修饰蛋白的多克隆抗体的方案。该方法使用迭代的减法和亲和纯化,使用严格的洗涤去除识别未修饰蛋白和含有修饰氨基酸的低序列复杂度表位的抗体。点印迹和 Western blot 分析用于评估抗体制备的特异性。该方法旨在克服一个常见的问题,即单轮减法和亲和纯化不足以获得修饰蛋白特异性的抗体制备。完整的一轮抗体纯化和特异性测试需要 6 天的不连续时间。

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