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数字PCR及荧光定量PCR测定豆乳饮料转基因成分分析

Yanbin Zhang,Libin Jing,Zhihui Gao, Xiaona Zhao,Hongbo Zhang

Modern Food(2020)

Cited 1|Views5
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Abstract
研究将转基因启动子CaMV35s、终止子NOS基因作为靶标,内标选择大豆内源基因Lectin,分别采用微滴式数字PCR及实时荧光PCR对标准品转基因大豆进行检测,实测20批次豆乳饮料转基因成份.结果显示,与实时荧光PCR相比,微滴式数字PCR对转基因筛查浓度检测低限、含量低限均较低,分别为0.04 ng/反应、0.05%,与欧盟转基因标识阈值要求符合.20批次样品中有16批次经过不同平台检测结果为阴性,1批次为阳性,3批次经过数字PCR检测获得准确结果,表明该检测技术能对实时荧光PCR起到辅助检测作用.
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