卡那霉素A酶联适配体检测方法研究  被引量:8

Development of Enzyme-linked Aptamer Assay for Detection of Kanamycin A

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作  者:刘信嘉 江颖妍 李美英 王弘 刘英菊[2] 卢蓝蓝 孙远明 雷红涛 

机构地区:[1]广东省食品质量安全重点实验室/农业部农产品贮藏质量安全风险评价重点实验室,广州510642 [2]华南农业大学理学院生物材料研究所,广州510642

出  处:《分析化学》2013年第9期1428-1433,共6页Chinese Journal of Analytical Chemistry

基  金:行业公益(农业)项目(No.201003008-08);国家重大基础研究项目(No.2012CB720803);国家自然科学基金项目(No.21105030);广东省科技计划项目(No.2012A020100002)资助

摘  要:通过EDC法偶联辣根过氧化物酶(HRP)和卡那霉素A(Kanamycin,KaA)分子制备酶标记物,采用棋盘滴定法确定链霉亲和素(Streptavidin,SA)的包被浓度为8 mg/L,通过单因素实验优化了检测条件,建立了卡那霉素A酶联适配体检测(Enzyme-linked aptamer assay,ELAA)方法。本方法半抑制浓度(IC50)为2.2"g/L,检出限(LOD)为0.04"g/L,检测范围(IC20~IC80)为0.07~71.5"g/L,与结构类似物无明显交叉反应;对牛奶、猪肉、猪肝、鸡肉、蜂蜜样品加标回收率在78%~100%之间,平均相对标准偏差小于11.1%。本方法特异性强、灵敏度高,适用于食品中卡那霉素A的快速检测。The EDC method was employed to conjugate the kanamycin A(KaA) to horseradish peroxidase(HRP).The optimal coating concentration of streptavidin was 8 mg/L and that was determined by chequerboard titration.The optimized assay conditions were investigated by single-factor experiments.An enzyme-linked aptamer assay(ELAA) method was established for the determination of kanamycin A(KaA).The half inhibition concentration(IC50) of the proposed method was 2.2 μg/L,the limit of detection(LOD) was 0.04 μg/L,and the detection ranged from 0.07 μg/L to 71.5 μg/L,There were no conspicuous cross reactions with other structural analogues of KaA.The recovery in milk,pork,pork liver,chicken and honey samples was 78%-100% and the RSD was less than 11.1%.This method is specific and highly sensitive,suitable for the rapid detection of kaA in variable food samples.

关 键 词:单链DNA(ssDNA) 适配体 卡那霉素A 酶联适配体 

分 类 号:TS207.3[轻工技术与工程—食品科学]

 

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