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刘玉敏,梁占丽,李兆杰,徐成钢,魏玮,张玉春.基于虾类原肌球蛋白共同表位肽抗体的过敏原检测方法[J].食品安全质量检测学报,2017,8(10):3963-3968

基于虾类原肌球蛋白共同表位肽抗体的过敏原检测方法

Rapid detection of shrimp allergens based against the polyclonal antibodies of shrimp tropomyosin common peptide epitopes

投稿时间：2017-07-23 修订日期：2017-09-25

DOI：

中文关键词: 虾类过敏原酶联免疫法共同表位肽抗体

英文关键词:shrimp allergen ELISA common epitopes peptide antibody

基金项目:山东检验检疫局科研计划项目(SK201615)、国家质量监督检验检疫总局科研项目(2015IK204)

作者	单位
刘玉敏	威海出入境检验检疫局
梁占丽	威海出入境检验检疫局
李兆杰	威海出入境检验检疫局
徐成钢	威海出入境检验检疫局
魏玮	威海出入境检验检疫局
张玉春	威海出入境检验检疫局

Author	Institution
LIU Yu-Min	Weihai Entry-Exit Inspection and Quarantine Bureau
LIANG Zhan-Li	Weihai Entry-Exit Inspection and Quarantine Bureau
LI Zhao-Jie	Weihai Entry-Exit Inspection and Quarantine Bureau
XU Cheng-Gang	Weihai Entry-Exit Inspection and Quarantine Bureau
WEI Wei	Weihai Entry-Exit Inspection and Quarantine Bureau
ZHANG Yu-Chun	Weihai Entry-Exit Inspection and Quarantine Bureau

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中文摘要:

目的建立一种能够同时检测多种虾原肌球蛋白的方法。方法通过合成不同虾类的共同表位肽, 制备能够识别多种虾类原肌球蛋白的共同表位肽多克隆抗体, 建立快速灵敏的虾类原肌球蛋白酶联免疫检测方法。结果该检测方法在4.79~1400 ng/mL的浓度范围内线性关系良好, 其线性回归方程为Y=-19.083X+ 98.303(R2=0.9813), 最低检出限(IC10)为1.85 ng/mL; 样品加标回收率在94.37%~103.45%之间; 该检测方法与软体动物的原肌球蛋白有交叉反应, 与鱼肉蛋白、牛奶、花生蛋白等无交叉反应; 批内变异系数为3.4%~9.1%, 板间变异系数为12.9%~19.6%, 贮藏试验显示该酶联免疫试剂盒可以在4 ℃下保存6个月以上, 能够应用于食品中虾类过敏原的检测。结论采用共同表位抗体, 成功建立了基于酶联免疫的过敏原检测方法。

英文摘要:

Objective To establish a method for simultaneous determination of various shrimp tropomyosins. Methods By synthesis of common peptide epitopes from different kinds of shrimp, polyclonal antibodies were produced which could identify a variety of shrimp tropomyosins. A rapid and sensitive ELISA method was established for the detection of shrimp tropomyosins. Results The method had a good linear relationship in the range of 4.79~1400 ng/mL, and the linear regression equation was Y=-19.083X+98.303(R2=0.9813). The limit of detection was 1.85 ng/mL(IC10), while the recovery rates were 94.37%~103.45%. The detection method was cross-responsive with invertebrate tropomyosin and had no cross reaction with fish protein, milk, and peanut protein. The coefficients of variation of the batch were 3.4%~9.1%, and the coefficients of variation of the plates were 12.9%~19.6%. The storage test showed that the ELISA kit could be stored more than 6 months at 4 ℃, which could be applied for the detection of shrimp allergens in food. Conclusion A simultaneous detection method of a variety of shrimp tropomyosins is establised successfully based on ELISA using common peptide epitopes.

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