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抗异丙威单克隆抗体的制备及其在免疫层析试纸条检测中的应用

Preparation of an anti-isoprocarb monoclonal antibody and its application in developing an immunochromatographic strip assay.

作者信息

Zhang Xiaoping, Liu Liqiang, Cui Gang, Song Shanshan, Kuang Hua, Xu Chuanlai

机构信息

State Key Laboratory of Food Science and Technology, Jiangnan University, Wuxi, People's Republic of China.

International Joint Research Laboratory for Biointerface and Biodetection, and School of Food Science and Technology, Jiangnan University, Wuxi, People's Republic of China.

出版信息

Biomed Chromatogr. 2019 Nov;33(11):e4660. doi: 10.1002/bmc.4660. Epub 2019 Aug 27.

Abstract

In this study, a carboxyl group was introduced into the isoprocarb molecule to obtain an isoprocarb hapten, which was then coupled with a protein to obtain an artificial antigen. Three monoclonal antibody cell lines, 1D11, 6E6 and 1B5, were finally obtained by mouse immunization, cell fusion and subcloning, and the antibody produced by cell line 1B5 had the best affinity and sensitivity. The monoclonal antibody was highly sensitive and specific for isoprocarb, with an IC of 2.09 ng/ml and a cross-reactivity rate of <0.21%. By optimizing the indirect competitive (ic)-ELISA, the optimal conditions were determined to be pH 7.4, 0% methanol and 0.8% NaCl, the limit of detection value was 0.23 ng/ml, and the linear range of the ic-ELISA was 0.46-9.62 ng/ml. The recovery rate of the isoprocarb cucumber sample was 97-99% for the ic-ELISA method. In addition, we successfully developed an immunochromatographic test strip for the detection of isoprocarb residues. The cutoff values in phosphate-buffered saline and cucumber extract were 10 and 25 ng/ml, respectively. Both methods met the requirements for isoprocarb residue detection in agricultural products, and can be used for semiquantitative and qualitative analysis of isoprocarb in vegetables.

摘要

本研究在异丙威分子中引入羧基得到异丙威半抗原,将其与蛋白质偶联获得人工抗原。通过小鼠免疫、细胞融合及亚克隆,最终获得3株单克隆抗体细胞株1D11、6E6和1B5,其中1B5细胞株产生的抗体亲和力和灵敏度最佳。该单克隆抗体对异丙威具有高灵敏度和特异性,IC为2.09 ng/ml,交叉反应率<0.21%。通过优化间接竞争(ic)-ELISA,确定最佳条件为pH 7.4、0%甲醇和0.8%氯化钠,ic-ELISA的检测限为0.23 ng/ml,线性范围为0.46 - 9.62 ng/ml。ic-ELISA法检测异丙威黄瓜样品的回收率为97 - 99%。此外,成功研制了一种检测异丙威残留的免疫层析试纸条,在磷酸盐缓冲液和黄瓜提取物中的截断值分别为10和25 ng/ml。两种方法均满足农产品中异丙威残留检测要求,可用于蔬菜中异丙威的半定量和定性分析。

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