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利用抗独特型骆驼纳米抗体的噬菌体介导竞争性化学发光免疫分析法检测Cry1Ab毒素

Phage-Mediated Competitive Chemiluminescent Immunoassay for Detecting Cry1Ab Toxin by Using an Anti-Idiotypic Camel Nanobody.

作者信息

Qiu Yulou, Li Pan, Dong Sa, Zhang Xiaoshuai, Yang Qianru, Wang Yulong, Ge Jing, Hammock Bruce D, Zhang Cunzheng, Liu Xianjin

机构信息

Laboratory for Food Quality and Safety-State Key Laboratory Cultivation Base of Ministry of Science and Technology,Key Laboratory of Control Technology and Standard for Agro-product Safety and Quality (Ministry of Agriculture), Institute of Food Safety and Nutrition, Jiangsu Academy of Agricultural Sciences , Nanjing 210014, China.

School of Horticulture and Plant Protection, Yangzhou University , Yangzhou 225009, China.

出版信息

J Agric Food Chem. 2018 Jan 31;66(4):950-956. doi: 10.1021/acs.jafc.7b04923. Epub 2018 Jan 22.

Abstract

Cry toxins have been widely used in genetically modified organisms for pest control, raising public concern regarding their effects on the natural environment and food safety. In this work, a phage-mediated competitive chemiluminescent immunoassay (c-CLIA) was developed for determination of Cry1Ab toxin using anti-idiotypic camel nanobodies. By extracting RNA from camels' peripheral blood lymphocytes, a naive phage-displayed nanobody library was established. Using anti-Cry1Ab toxin monoclonal antibodies (mAbs) against the library for anti-idiotypic antibody screening, four anti-idiotypic nanobodies were selected and confirmed to be specific for anti-Cry1Ab mAb binding. Thereafter, a c-CLIA was developed for detection of Cry1Ab toxin based on anti-idiotypic camel nanobodies and employed for sample testing. The results revealed a half-inhibition concentration of developed assay to be 42.68 ± 2.54 ng/mL, in the linear range of 10.49-307.1 ng/mL. The established method is highly specific for Cry1Ab recognition, with negligible cross-reactivity for other Cry toxins. For spiked cereal samples, the recoveries of Cry1Ab toxin ranged from 77.4% to 127%, with coefficient of variation of less than 9%. This study demonstrated that the competitive format based on phage-displayed anti-idiotypic nanobodies can provide an alternative strategy for Cry toxin detection.

摘要

Cry毒素已广泛应用于转基因生物的害虫防治,这引发了公众对其对自然环境和食品安全影响的关注。在本研究中,开发了一种噬菌体介导的竞争性化学发光免疫分析方法(c-CLIA),用于使用抗独特型骆驼纳米抗体测定Cry1Ab毒素。通过从骆驼外周血淋巴细胞中提取RNA,建立了一个原始的噬菌体展示纳米抗体文库。使用抗Cry1Ab毒素单克隆抗体(mAbs)针对该文库进行抗独特型抗体筛选,选择了四种抗独特型纳米抗体,并证实它们对与抗Cry1Ab mAb结合具有特异性。此后,基于抗独特型骆驼纳米抗体开发了一种用于检测Cry1Ab毒素的c-CLIA,并用于样品检测。结果显示,所开发分析方法的半抑制浓度为42.68±2.54 ng/mL,线性范围为10.49-307.1 ng/mL。所建立的方法对Cry1Ab的识别具有高度特异性,对其他Cry毒素的交叉反应可忽略不计。对于加标的谷物样品,Cry1Ab毒素的回收率在77.4%至127%之间,变异系数小于9%。本研究表明,基于噬菌体展示抗独特型纳米抗体的竞争模式可为Cry毒素检测提供一种替代策略。

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