转基因苜蓿J101、J163和KK179事件特异性qPCR检测方法的开发。

Q1 Biochemistry, Genetics and Molecular Biology Biomolecular Detection and Quantification Pub Date : 2019-03-01 DOI:10.1016/j.bdq.2018.12.001
Patrick Guertler , Lutz Grohmann , Heike Naumann , Melanie Pavlovic , Ulrich Busch
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引用次数: 8

摘要

自2005年以来,转基因苜蓿已获准在几个国家种植。另一方面,不允许在欧盟种植或出口,因此既没有经过认证的参考材料,也没有针对特定事件的官方检测方法。因此,基于专利序列信息,开发了针对苜蓿基因组的连接序列和相应事件J101、J163和KK179的转基因插入物的事件特异性实时PCR检测方法。新开发的质粒被用作分析优化和内部验证的参考材料。质粒标准品使用数字液滴PCR进行定量,LOD95%,PCR效率、稳健性和特异性使用实时PCR进行测定。观察到每个PCR反应10个拷贝的LOD95%,并且实现了95-97%的PCR效率。应用不同的实时PCR仪器和PCR条件来测试使用浓度为每μL 30个拷贝的DNA对每个转基因苜蓿事件进行测定的稳健性。所有重复均为阳性,与仪器或PCR条件无关。使用来自不同转基因作物的认证参考材料以及三个事件的参考材料的DNA进行特异性实验测试。在任何测定中均未观察到非特异性扩增信号。验证结果符合欧洲转基因实验室网络的“转基因检测分析方法的最低性能要求”。此外,还进行了实验室间比较研究,以显示这些方法的可转移性和适用性,并验证分析性能参数。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Development of event-specific qPCR detection methods for genetically modified alfalfa events J101, J163 and KK179

Genetically modified alfalfa is authorized for cultivation in several countries since 2005. On the other hand, cultivation in or export to the European Union is not allowed and thus neither certified reference material nor official event-specific detection methods are available. Therefore, based on patent sequence information, event-specific real-time PCR detection methods targeting the junction sequence of the alfalfa genome and the transgenic insert of the respective events J101, J163 and KK179 were developed. Newly developed plasmids were used as reference material for assay optimization and in-house validation. Plasmid standards were quantified using digital droplet PCR and LOD95%, PCR efficiency, robustness and specificity of the assays were determined using real-time PCR. A LOD95% of 10 copies per PCR reaction was observed and PCR efficiencies of 95–97 % were achieved. Different real-time PCR instruments and PCR conditions were applied to test for robustness of the assays using DNA at a concentration of 30 copies per μL for each gm alfalfa event. All replicates were positive independent of the instrument or the PCR condition. DNA from certified reference material of different genetically modified crops as well as reference materials of the three events was used to experimentally test for specificity. No unspecific amplification signal was observed for any of the assays. Validation results were in line with the “Minimum Performance Requirements for Analytical Methods of GMO Testing” of the European Network of GMO Laboratories. Furthermore, an inter-laboratory comparison study was conducted to show the transferability and applicability of the methods and to verify the assay performance parameters.

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来源期刊
Biomolecular Detection and Quantification
Biomolecular Detection and Quantification Biochemistry, Genetics and Molecular Biology-Biochemistry
CiteScore
14.20
自引率
0.00%
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0
审稿时长
8 weeks
期刊最新文献
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