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固相夹心酶联免疫吸附测定的免疫化学

The immunochemistry of solid-phase sandwich enzyme-linked immunosorbent assays.

作者信息

Butler J E, Peterman J H, Suter M, Dierks S E

出版信息

Fed Proc. 1987 Jun;46(8):2548-56.

PMID:3595892
Abstract

Multivalent antigens (Ags) such as membrane proteins can be quantitated by using sandwich enzyme-linked immunosorbent assays (ELISAs), which typically show sensitivity from 0.1 to 50 ng/ml. The percentage of antigen that binds in the log-log linear region reflects the affinity of the capture antibody (CAb), and the range of linearity for assays conducted with a particular CAb is proportional to the antibody (Ab) concentration. The sandwich ELISA titration plot reflects the actual amount of Ag bound when asymmetrical configurations are used; steric hindrance that occurs with certain symmetrical configurations, especially when enzyme-Ab conjugates of greater than or equal to 10(6) daltons are used, can alter this relationship. Monoclonal CAbs bind less Ag than polyclonal CAbs. Immobilization of monoclonal CAbs by using a modified avidin-biotin system can result in greater antigen capture capacity (AgCC) than when the Abs are directly adsorbed on plastic. Adsorption of proteins on polystyrene is noncovalent and proportional to the amount added for up to 150 ng/200 microliter in a microtiter well. Adsorption can result in substantial loss of antigenic or antibody activity. Desorption is continuous at a low level and can negatively influence the results of an immunoassay. Data from microtiter sandwich ELISAs can be readily acquired and analyzed by using a computer-based analysis system (ELISANALYSIS) written for the IBM PC. This analytical system considers the immunochemical principles of sandwich ELISAs predicted theoretically and demonstrated empirically.

摘要

多价抗原(如膜蛋白)可通过夹心酶联免疫吸附测定(ELISA)进行定量,其灵敏度通常为0.1至50 ng/ml。在对数-对数线性区域结合的抗原百分比反映了捕获抗体(CAb)的亲和力,使用特定CAb进行测定的线性范围与抗体(Ab)浓度成正比。夹心ELISA滴定图反映了使用不对称构型时结合的抗原实际量;某些对称构型会出现空间位阻,尤其是当使用大于或等于10(6)道尔顿的酶-抗体缀合物时,会改变这种关系。单克隆CAb比多克隆CAb结合的抗原少。使用改良的抗生物素蛋白-生物素系统固定单克隆CAb比将抗体直接吸附在塑料上可产生更大的抗原捕获能力(AgCC)。蛋白质在聚苯乙烯上的吸附是非共价的,在微量滴定孔中,吸附量与添加量成正比,最高可达150 ng/200微升。吸附可能导致抗原或抗体活性大量丧失。解吸在低水平上持续进行,会对免疫测定结果产生负面影响。微量滴定夹心ELISA的数据可通过使用为IBM PC编写的基于计算机的分析系统(ELISANALYSIS)轻松获取和分析。该分析系统考虑了理论上预测并经实验证明的夹心ELISA的免疫化学原理。

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