A Specific Real-Time Quantitative PCR Detection System for Event MON810 in Maize YieldGard® Based on the 3′-Transgene Integration Sequence

被引:1
作者
Marta Hernández
Maria Pla
Teresa Esteve
Salomé Prat
Pere Puigdomènech
Alejandro Ferrando
机构
[1] Instituto de Biología Molecular de Barcelona (IBMB)-Consejo Superior de Investigaciones Científicas (CSIC),
来源
Transgenic Research | 2003年 / 12卷
关键词
GMO; MON810 event; real-time PCR; TAIL-PCR; TaqMan;
D O I
暂无
中图分类号
学科分类号
摘要
The increasing presence of transgenic plant derivatives in a wide range of animal and human consumables has provoked in western Europe a strong demand for appropriate detection methods to evaluate the existence of transgenic elements. Among the different techniques currently used, the real-time quantitative PCR is a powerful technology well adapted to the mandatory labeling requirements in the European Union (EU). The use of transgene flanking genomic sequences has recently been suggested as a means to avoid ambiguous results both in qualitative and quantitative PCR-based technologies. In this study we report the identification of genomic sequences adjacent to the 3′-integration site of event MON810 in transgenic maize. This genetically modified crop contains transgene sequences leading to ectopic expression of a synthetic CryIA(b) endotoxin which confers resistance to lepidopteran insects especially against the European corn borer. The characterization of the genome–transgene junction sequences by means of TAIL-PCR has facilitated the design of a specific, sensitive and accurate quantification method based on TaqMan chemistry. Cloning of event MON810 3′-junction region has also allowed to compare the suitability of plasmid target sequences versus genomic DNA obtained from certified reference materials (CRMs), to prepare standard calibration curves for quantification.
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页码:179 / 189
页数:10
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