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通过实时相互作用分析研究双特异性多价抗体以开发抗原抑制酶联免疫吸附测定法。

Bispecific multivalent antibody studied by real-time interaction analysis for the development of an antigen-inhibition enzyme-linked immunosorbent assay.

作者信息

Reinartz H W, Quinn J G, Zänker K, O'Kennedy R

机构信息

Institute of Immunology, Universität Witten/Herdecke, Germany.

出版信息

Analyst. 1996 Jun;121(6):767-71. doi: 10.1039/an9962100767.

Abstract

A bispecific antibody with specificities for both 7-hydroxycoumarin (7-OHC) and alkaline phosphatase (AP) was produced by chemically cross-linking two parental polyclonal antibodies. Real-time interaction analysis of the bispecific multivalent antibody (bsMAb) was performed using BIAcore, a surface plasmon resonance (SPR)-based biosensor, in order to confirm its bispecific nature. A 7-OHC-BSA conjugate was covalently immobilized to a dextran matrix to serve as the reaction surface and unconjugated bovine serum albumin (BSA) was immobilized on to a separate dextran matrix as a control surface. Immunoaffinity-purified bsMAb, parental anti-7-OHC antibody and AP were injected over both surfaces. The bsMAb was shown to bind both antigens, 7-OHC and AP, simultaneously. Comparison of the ratio of mass bound for bsMAb and AP (5:1) with the ratio of the molecular masses of bsMAb (approximately 300 kDa) and AP (85 kDa) (3.5:1) suggests that most of the bsMAb species possess both specificities. The bsMAb was employed in a one-step antigen-inhibition ELISA for the detection of 7-OHC. The assay was compared with a conventional ELISA approach employing an AP-labelled secondary antibody. The bispecific antibody approach proved to be faster and more sensitive, with a detection limit of 6 ng ml-1 as compared with approximately 50 ng ml-1 for the conventional approach. The assay was used for the quantification of free and total 7-OHC in urine samples from two healthy volunteers who had been administered coumarin. The accuracy and precision of the assay were assessed. The bispecific antibody-based assay gave similar results, accuracy and precision, but proved to be far more sensitive (limit of determination 6 ng ml-1 for total 7-OHC). It is concluded that real-time interaction analysis using BIAcor provides a rapid method for the evaluation of the bsMAb and it was verified that the bispecific product formed by chemical cross-linking of two parental antibodies offers a simple alternative for the development of a highly sensitive ELISA.

摘要

通过化学交联两种亲本多克隆抗体制备了一种对7-羟基香豆素(7-OHC)和碱性磷酸酶(AP)均具有特异性的双特异性抗体。使用基于表面等离子体共振(SPR)的生物传感器BIAcore对双特异性多价抗体(bsMAb)进行实时相互作用分析,以确认其双特异性性质。将7-OHC-BSA缀合物共价固定在葡聚糖基质上作为反应表面,并将未缀合的牛血清白蛋白(BSA)固定在单独的葡聚糖基质上作为对照表面。将免疫亲和纯化的bsMAb、亲本抗7-OHC抗体和AP注射到两个表面上。结果表明,bsMAb能同时结合两种抗原,即7-OHC和AP。bsMAb与AP的结合质量比(5:1)与bsMAb(约300 kDa)和AP(85 kDa)的分子量比(3.5:1)的比较表明,大多数bsMAb物种具有两种特异性。将bsMAb用于一步法抗原抑制ELISA检测7-OHC。将该检测方法与采用AP标记二抗的传统ELISA方法进行比较。结果证明,双特异性抗体方法更快、更灵敏,检测限为6 ng/ml,而传统方法约为50 ng/ml。该检测方法用于定量来自两名服用香豆素的健康志愿者尿液样本中的游离和总7-OHC。评估了该检测方法的准确性和精密度。基于双特异性抗体的检测方法给出了相似的结果、准确性和精密度,但证明灵敏度更高(总7-OHC的测定限为6 ng/ml)。结论是,使用BIAcor进行实时相互作用分析为评估bsMAb提供了一种快速方法,并且证实通过化学交联两种亲本抗体制备的双特异性产物为开发高灵敏度ELISA提供了一种简单的替代方法。

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