欢迎访问《食品安全质量检测学报》网站！

刘二龙,卢丽,吕英姿,蒋湘,张旺,林惠娇,郑高彬,唐婕,林学勤,秦焯敏.转基因苜蓿草J163品系特异性实时荧光PCR检测方法的建立[J].食品安全质量检测学报,2015,6(1):272-278

转基因苜蓿草J163品系特异性实时荧光PCR检测方法的建立

Establishing an event-specific real-time polymerase chain reaction detection method for genetically modified alfalfa events J163

投稿时间：2014-11-27 修订日期：2015-01-14

DOI：

中文关键词: 实时荧光PCR 转基因苜蓿J163 品系特异性

英文关键词:quantitative real-time PCR genetically modified alfalfa J163 event-specificity

基金项目:陕西省科学院应用基础专项 (2013K-12)

作者	单位
刘二龙	黄埔出入境检验检疫局
卢丽	广东出入境检验检疫局
吕英姿	黄埔出入境检验检疫局
蒋湘	黄埔出入境检验检疫局
张旺	广东出入境检验检疫局
林惠娇	黄埔出入境检验检疫局
郑高彬	黄埔出入境检验检疫局
唐婕	陕西省动物研究所
林学勤	黄埔出入境检验检疫局
秦焯敏	黄埔出入境检验检疫局

Author	Institution
LIU Er-Long	Huangpu Entry-Exit Inspection and Quarantine Bureau
LU Li	Guangdong Entry–Exit Inspection and Quarantine Bureau
LV Ying-Zi	Huangpu Entry-Exit Inspection and Quarantine Bureau
JIANG Xiang	Huangpu Entry-Exit Inspection and Quarantine Bureau
ZHANG Wang	Guangdong Entry–Exit Inspection and Quarantine Bureau
LIN Hui-Jiao	Huangpu Entry-Exit Inspection and Quarantine Bureau
ZHENG Gao-Bin	Huangpu Entry-Exit Inspection and Quarantine Bureau
TANG Jie	Shaanxi Institute of Zoology
LIN Xue-Qin	Huangpu Entry-Exit Inspection and Quarantine Bureau
QIN Chao-Min	Huangpu Entry-Exit Inspection and Quarantine Bureau

摘要点击次数: 2197

全文下载次数: 1763

中文摘要:

目的建立针对我国农业部未颁发农业转基因生物安全证书的转基因苜蓿草品系J163品系特异性实时荧光(Polymerase Chain Reaction，PCR)检测方法。方法利用TaqMan实时荧光PCR(real-time PCR)技术, 根据转基因苜蓿草品系J163 5’端外源插入片段P-eFMV与苜蓿草基因组DNA之间的邻接区序列设计引物和探针, 建立了转基因苜蓿草J163品系特异性实时荧光PCR检测方法, 并对本方法的特异性、灵敏度及可重复性进行了测定。结果建立的检测方法特异于转基因苜蓿草J163成分检测, 检测最低DNA浓度为(1imit of detection, LOD)为15 pg, 相当于9拷贝转基因苜蓿草J163基因组DNA, 重复性试验显示, 其标准偏差(Standard deviation, SD)和相对标准偏差(relative standard deviation, RSD)均在可接受范围内。结论本研究建立的转基因苜蓿草J163品系特异性实时荧光PCR检测方法特异性好, 灵敏度高, 能够快速、准确、稳定地对转基因苜蓿草J163成分进行检测分析。

英文摘要:

Objective To establish a real-time PCR detection method for genetically modified (GM) Roundup Ready alfalfa events J163, which has not been authorized by the Ministry of Agriculture of China. Method The specific primer pairs and probe based on the 5’junction sequence spanning the alfalfa DNA and inserted P-eFMV fragment of J163 were designed and then the real-time PCR detection system was established. The specificity, sensitivity and repeatability were analyzed. Results The real-time PCR method was specific for GM alfalfa J163 detection, the limit of detection(LOD) were 15 pg J163 genomic DNA or 10 copies of al-falfa J163 haploid genomic DNA. Repeatability of the established event-specific real-time PCR method for GM alfalfa J163 was assessed and the standard deviation (SD) and the relative standard deviation (RSD) were all in the acceptable range. Conclusion The established event-specific quantitative real-time PCR method for GM alfalfa J163 detection has a high specificity and a good sensitivity, and is suitable for quantification of J163 samples quickly and accurately.

查看全文查看/发表评论下载PDF阅读器