Highly Sensitive GMO Detection Using Real-Time PCR with a Large Amount of DNA Template: Single-Laboratory Validation

Current genetically modified organism (GMO) detection methods allow for sensitive detection. However, a further increase in sensitivity will enable more efficient testing for large grain samples and reliable testing for processed foods. In this study, we investigated real-time PCR-based GMO detectio...

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Bibliographic Details
Published inJournal of AOAC International Vol. 101; no. 2; pp. 507 - 514
Main Authors Mano, Junichi, Hatano, Shuko, Nagatomi, Yasuaki, Futo, Satoshi, Takabatake, Reona, Kitta, Kazumi
Format Journal Article
LanguageEnglish
Published England Oxford University Press 01.03.2018
Subjects
DNA Primers - genetics
DNA, Plant - chemistry
Edible Grain - genetics
Food, Genetically Modified
Genetic aspects
Genetically modified organisms
Identification and classification
Limit of Detection
Methods
Plants, Genetically Modified - genetics
Polymerase chain reaction
Real-Time Polymerase Chain Reaction - methods
Zea mays - genetics
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Summary:Current genetically modified organism (GMO) detection methods allow for sensitive detection. However, a further increase in sensitivity will enable more efficient testing for large grain samples and reliable testing for processed foods. In this study, we investigated real-time PCR-based GMO detection methods using a large amount of DNA template. We selected target sequences that are commonly introduced into many kinds of GM crops, i.e., 35S promoter and nopaline synthase (NOS) terminator. This makes the newly developed method applicable to a wide range of GMOs, including some unauthorized ones. The estimated LOD of the new method was 0.005% of GM maize events; to the best of our knowledge, this method is the most sensitive among the GM maize detection methods for which the LOD was evaluated in terms of GMO content. A 10-fold increase in the DNA amount as compared with the amount used under common testing conditions gave an approximately 10-fold reduction in the LOD without PCR inhibition. Our method is applicable to various analytical samples, including processed foods. The use of other primers and fluorescence probes would permit highly sensitive detection of various recombinant DNA sequences besides the 35S promoter and NOS terminator.
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ISSN:1060-3271
1944-7922
DOI:10.5740/jaoacint.17-0197