作物学报 ›› 2023, Vol. 49 ›› Issue (7): 1818-1828.doi: 10.3724/SP.J.1006.2023.23048
常丽娟1(), 梁晋刚2,*(), 宋君1, 刘文娟1, 付成平3, 代晓航1, 王东1, 魏超1, 熊梅1
CHANG Li-Juan1(), LIANG Jing-Gang2,*(), SONG Jun1, LIU Wen-Juan1, FU Cheng-Ping3, DAI Xiao-Hang1, WANG Dong1, WEI Chao1, XIONG Mei1
摘要:
转基因玉米ND207是中国农业大学研发的转mCry1Ab和mCry2Ab基因的抗虫玉米, 本研究的目的是建立ND207转化事件特异性定性PCR检测方法。根据研发者提供的引物进行PCR扩增, PCR产物测序分析, 获得了5'端旁侧序列262 bp, 包括109 bp的载体序列和153 bp的玉米基因组序列, 3'端旁侧序列316 bp, 包括76 bp的载体序列和240 bp的玉米基因组序列。针对两端旁侧序列设计14条引物, 组成25对引物组合进行引物筛选, 选中3'端一对最佳引物优化PCR反应体系及反应条件, 建立ND207的转化事件特异性定性PCR检测方法, PCR产物片段大小为166 bp。经过测试, 该方法的检出限为0.1%, 相当于20个拷贝的ND207特异分子片段。国内8家转基因生物安全检测机构对本方法进行了特异性测试、检出限测试和再现性测试, 循环验证报告显示: 该方法符合国家标准方法的各项要求, 可在检测行业推广应用。ND207转化事件特异性定性PCR检测方法的建立, 为我国ND207及其衍生品系的安全监管提供技术支撑。
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