Simple Determination of Affinity Constants of Antibodies by Competitive Immunoassays

IF 2.3 Q3 BIOCHEMICAL RESEARCH METHODS
Janina Fischer, Jan Ole Kaufmann, Michael G. Weller
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Abstract

The affinity constant, also known as the equilibrium constant, binding constant, equilibrium association constant, or the reciprocal value, the equilibrium dissociation constant (Kd), can be considered as one of the most important characteristics for any antibody–antigen pair. Many methods based on different technologies have been proposed and used to determine this value. However, since a very large number of publications and commercial datasheets do not include this information, significant obstacles in performing such measurements seem to exist. In other cases where such data are reported, the results have often proved to be unreliable. This situation may indicate that most of the technologies available today require a high level of expertise and effort that does not seem to be available in many laboratories. In this paper, we present a simple approach based on standard immunoassay technology that is easy and quick to perform. It relies on the effect that the molar IC50 approaches the Kd value in the case of infinitely small concentrations of the reagent concentrations. A two-dimensional dilution of the reagents leads to an asymptotic convergence to Kd. The approach has some similarity to the well-known checkerboard titration used for the optimization of immunoassays. A well-known antibody against the FLAG peptide, clone M2, was used as a model system and the results were compared with other methods. This approach could be used in any case where a competitive assay is available or can be developed. The determination of an affinity constant should belong to the crucial parameters in any quality control of antibody-related products and assays and should be mandatory in papers using immunochemical protocols.
用竞争性免疫测定法简单测定抗体的亲和常数
亲和力常数,又称平衡常数、结合常数、平衡关联常数,或其倒数值--平衡解离常数(Kd),可被视为任何抗体-抗原配对的最重要特征之一。许多基于不同技术的方法已被提出并用于确定该值。然而,由于大量的出版物和商业数据表都不包含这一信息,因此在进行此类测量时似乎存在很大的障碍。在报告了此类数据的其他情况下,结果往往被证明是不可靠的。这种情况可能表明,当今的大多数技术都需要高水平的专业知识和努力,而许多实验室似乎并不具备这种能力。在本文中,我们介绍了一种基于标准免疫测定技术的简单方法,该方法简便快捷。它依赖于在试剂浓度无限小的情况下摩尔 IC50 接近 Kd 值的效应。试剂的二维稀释会导致向 Kd 的渐近收敛。这种方法与著名的用于优化免疫测定的棋盘滴定法有些相似。我们使用了一种著名的 FLAG 肽抗体克隆 M2 作为模型系统,并将结果与其他方法进行了比较。这种方法适用于有竞争性检测方法或可以开发竞争性检测方法的任何情况。亲和力常数的测定应属于抗体相关产品和检测质量控制的关键参数,在使用免疫化学方案的论文中也应强制使用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Methods and Protocols
Methods and Protocols Biochemistry, Genetics and Molecular Biology-Biochemistry, Genetics and Molecular Biology (miscellaneous)
CiteScore
3.60
自引率
0.00%
发文量
85
审稿时长
8 weeks
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