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Preparation and Identification of Monoclonal Antibody against Abrin-a

机译:抗Abrin-a单克隆抗体的制备与鉴定

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BALB/c mice were immunized four times with formalin-prepared abrin-a. Using the polyethylene glycol method, immunized splenocytes were isolated and fused with SP2/0 cells. An indirect ELISA was established and used to detect positive clones secreting monoclonal antibodies (mAbs) against abrin-a. After analysis, three hybridoma clones secreting IgG-subtype mAbs were obtained. The antibodies were purified from the hybridoma growth medium using protein A or G affinity chromatography. Western blot analysis was used to analyze the antigenic epitopes on abrin-a recognized by the mAbs. The mAbs were specific for abrin-a, with no detectable cross-reactivity with several homologous toxins and associated agglutinins. Sandwich ELISA was then developed using these mAbs, which had a detection limit for abrin-a of 7.8 ng/mL.
机译:BALB / c小鼠用福尔马林制备的abrin-a免疫四次。使用聚乙二醇方法,分离免疫的脾细胞并与SP2 / 0细胞融合。建立了间接ELISA,并用于检测分泌抗abrin-a单克隆抗体(mAb)的阳性克隆。经过分析,获得了分泌IgG亚型mAb的三个杂交瘤克隆。使用蛋白A或G亲和层析从杂交瘤生长培养基中纯化抗体。使用蛋白质印迹分析来分析单克隆抗体识别的abrin-a上的抗原表位。 mAb对abrin-a具有特异性,与几种同源毒素和相关凝集素没有可检测到的交叉反应性。然后,使用这些mAb进行了夹心ELISA,对abrin-a的检出限为7.8 ng / mL。

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