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Identification of a common Ara h 3 epitope recognized by both the capture and the detection monoclonal antibodies in an ELISA detection kit

机译:ELISA检测试剂盒中捕获和检测单克隆抗体均可识别的常见Ara h 3表位的鉴定

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摘要

Allergy to peanuts has become a common and severe problem, especially in westernized countries. In this study, we evaluated the target and epitope specificity of the capture and detection mouse monoclonal antibodies (mAbs) used in a commercial peanut allergen detection platform. We first identified the target of these antibodies as Ara h 3 and then used an overlapping peptide array of Ara h 3 to determine the antibody-binding epitopes. Further amino acids critical for the binding via alanine substitutions at individual amino acid residues within the epitope were mapped. Finally, inhibition ELISA and inhibition immunoblotting using a recombinant Ara h 3 protein were performed to confirm these results. Surprisingly, the capture and detection mAbs showed identical binding characteristics and were presumed to represent two isolates of the same clone, a notion supported by both isoelectric focusing electrophoresis and Liquid chromatography–mass spectrometry experiments. The simultaneous binding of a pair of identical mAbs to an individual allergen such as Ara h3 is attributed to the multivalency of the analyte and has implications for developing diagnostic assays for additional multimeric allergens.
机译:花生过敏已成为普遍而严重的问题,尤其是在西方国家。在这项研究中,我们评估了在商业花生过敏原检测平台中使用的捕获和检测小鼠单克隆抗体(mAb)的靶标和表位特异性。我们首先将这些抗体的靶标定为Ara h 3,然后使用Ara h 3的重叠肽阵列确定抗体结合表位。对在表位内各个氨基酸残基上通过丙氨酸取代的结合至关重要的其他氨基酸进行了图谱。最后,使用重组Ara h 3蛋白进行抑制ELISA和抑制免疫印迹以证实这些结果。出乎意料的是,捕获和检测单克隆抗体显示出相同的结合特性,并被认为代表了同一克隆的两个分离株,这一概念由等电聚焦电泳和液相色谱-质谱实验共同支持。一对相同的mAb与单个变应原(例如Ara h3)的同时结合可归因于分析物的多价态,对开发其他多聚体变应原的诊断检测方法具有重要意义。

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