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Immunosorbent analysis of ricin contamination in milk using colorimetric, chemiluminescent and electrochemiluminescent detection.

机译:使用比色法,化学发光法和电化学发光法检测牛奶中蓖麻毒素的免疫吸附剂。

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摘要

Analytical methodology to detect active ricin in food matrices is important because of the potential use of foodborne ricin as a terrorist weapon. Monoclonal antibodies (mAbs) that bind ricin were used as both capture and detection ligands in sandwich enzyme-linked immunosorbent assay (ELISA) and electrochemiluminescent (ECL) immunosorbent assays. ELISA employed two types of substrate for colorimetric or chemiluminescent detection. Although both fat content and protein content of samples influenced the recovery of ricin, the lower limit of detection (LOD) in ELISA and ECL systems permitted detection of 0.1 ng/mL for milk samples containing 0-4% fat. The assay systems detect pure ricin- or crude ricin-containing castor extract, but do not significantly respond to isolated ricin chains, heat-denatured ricin or the related agglutinin, Ricinus communis agglutinin 1 (RCA-1). Using the standard 96-well-plate formats, the assays detect less than 0.01% of an adult human lethal dose in a typical serving of milk.
机译:检测食品基质中活性蓖麻毒素的分析方法很重要,因为食源性蓖麻毒素有可能被用作恐怖武器。结合蓖麻毒素的单克隆抗体(mAb)在夹心酶联免疫吸附测定(ELISA)和电化学发光(ECL)免疫吸附测定中用作捕获和检测配体。 ELISA采用两种类型的底物进行比色或化学发光检测。尽管样品中的脂肪含量和蛋白质含量均影响蓖麻毒素的回收率,但ELISA和ECL系统中的检测下限(LOD)允许对脂肪含量为0-4%的牛奶样品进行0.1 ng / mL的检测。该测定系统可检测纯蓖麻毒素或粗蓖麻毒素蓖麻提取物,但对分离的蓖麻毒素链,热变性的蓖麻毒素或相关凝集素Ricinus communis凝集素1(RCA-1)没有明显反应。使用标准的96孔板格式,该检测方法在典型的牛奶中检测不到成人致死剂量的0.01%。

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