基于免扩增高通量测序的转基因定量检测方法研究  

作　　者：李凯 付军 陈锐[3] 陈笑芸[4] 李亮 LI Kai;FU Jun;CHEN Rui;CHEN Xiaoyun;LI Liang(Institute of Quality Standard and Testing Technology for Agro-products,Chinese Academy of Agricultural Sciences,Beijing 100081,China;Maccura Biotech Co.,Ltd,Chengdu 610041,China;State Key Laboratory of Vegetable Biobreeding,Institute of Germplasm Resources and Biotechnology,Tianjin Academy of Agricultural Sciences,Tianjin 300192,China;Key Laboratory of Traceability for Agricultural Genetically Modified Organisms,Ministry of Agriculture and Rural Affairs,Zhejiang Academy of Agricultural Sciences,Hangzhou 310021,China)

机构地区：[1]中国农业科学院农业质量标准与检测技术研究所,北京100081 [2]迈克生物股份有限公司,成都610041 [3]天津市农业科学院种质资源与生物技术研究所,蔬菜生物育种全国重点实验室,天津300381 [4]浙江省农业科学院农产品质量安全与营养研究所,农业农村部农业转基因生物溯源重点实验室,杭州310021

出　　处：《生物技术进展》2024年第4期610-617,共8页Current Biotechnology

基　　金：农业农村部农业转基因生物溯源重点实验室开放课题(2022KF02);科技创新2030农业生物育种重大专项(2022ZD0402013);中国农业科学院科技创新工程(CAAS-ASTIP-IQSTAP-05);中国农业科学院研究所级工作任务(1610072023101)。

摘　　要：转基因定量检测在食品安全监管和消费者知情权保障中扮演着重要角色。当前,数字PCR方法被广泛认可为核酸精准定量的黄金标准,但缺乏与之相互验证的新型核酸定量技术,这在一定程度上限制了其应用。然而,近年来高通量测序技术的兴起为解决这一难题提供了新的可能性。尽管高通量测序技术主要用于核酸定性序列测定,但其在核酸定量领域的应用潜力尚未充分挖掘。以含有转基因T-NOS、P-35S、CP4-EPSPS和大豆内标准基因Lectin的质粒DNA标准物质为检测对象,采用免扩增建库的方法,比较了NGS、三代测序以及数字PCR定值的差异。结果表明,NGS测序结果与数字PCR结果存在显著性差异,这一发现突显了目前核酸定量技术中的挑战和需求。然而,值得注意的是,三代测序结果与数字PCR检测结果一致性良好,显示了其作为转基因核酸精准定量方法的潜力。这一发现为未来转基因产品标识阈值的制定提供了技术上的支撑和参考,为食品安全监管提供了新的技术途径。Quantitative GMO detection is essential for ensuring food safety and protecting consumer rights to information.Although digital PCR is currently considered the gold standard for accurate nucleic acid quantification,the lack of validated new quantification technologies limits its applications.However,the emergence of high-throughput sequencing has opened up new possibilities for solving this challenge.While high-throughput sequencing is primarily used for qualitative nucleic acid sequence determination,its potential for quantitative analysis has yet to be fully explored.In this study,plasmid DNA standard materials containing transgenic T-NOS,P-35S,CP4-EPSPS,and soybean housekeeping gene Lectin were used as the detection objects.The method of library construction without amplification was adopted to compare the differences between NGS,third-generation sequencing,and digital PCR quantification.The results showed significant differences between NGS sequencing results and digital PCR results,highlighting the challenges and demands in current nucleic acid quantitative analysis technologies.However,it is worth noting that the results of third-generation sequencing were consistent with the digital PCR detection results,demonstrating its potential as a precise method for quantifying transgenic nucleic acids.

关 键 词：质粒DNA 标准物质 测序技术 dPCR 

分 类 号：Q789[生物学—分子生物学]