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Multiplex Real-Time PCR-Based Detection and Quantification of Genetically Modified Maize Events Employing SYBR® Green I and Taqman® Chemistries


Affiliations
1 Division of Genomic Resources, Indian Council of Agricultural Research-National Bureau of Plant Genetic Resources, New Delhi 110 012, India
2 Department of Plant Science, School of Life Sciences, Bharathidasan University, Tiruchirappalli 620 024, India
 

Multiplexing in real-time PCR offers advantages over singleplex real-time PCR by saving time and re-sources. SYBR® Green I-based duplex and triplex re-al-time PCR assays targeting event-specific sequences of three genetically modified (GM) maize events, namely Bt11, Bt176 and MON89034, and taxon-specific endogenous Adh1 gene were developed to sim-ultaneously identify multiple events. Duplex real-time PCR assay based on TaqMan® chemistry targeting Bt176 event-specific sequence and Adh1 was also op-timized for quantification purpose. Limit of detection of developed assays was up to 0.05% and limit of quantification of the reported TaqMan® based real-time PCR was up to 0.5%.

Keywords

Dyes, Genetically Modified Maize, Gm De-Tection And Quantification, Multiplex Real-Time PCR, Pri-Mers and Probes.
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  • Multiplex Real-Time PCR-Based Detection and Quantification of Genetically Modified Maize Events Employing SYBR® Green I and Taqman® Chemistries

Abstract Views: 271  |  PDF Views: 83

Authors

Rajesh K. Bhoge
Division of Genomic Resources, Indian Council of Agricultural Research-National Bureau of Plant Genetic Resources, New Delhi 110 012, India
Rashmi Chhabra
Division of Genomic Resources, Indian Council of Agricultural Research-National Bureau of Plant Genetic Resources, New Delhi 110 012, India
Monika Singh
Division of Genomic Resources, Indian Council of Agricultural Research-National Bureau of Plant Genetic Resources, New Delhi 110 012, India
Muthukrishnan Sathiyabama
Department of Plant Science, School of Life Sciences, Bharathidasan University, Tiruchirappalli 620 024, India
Gurinderjit Randhawa
Division of Genomic Resources, Indian Council of Agricultural Research-National Bureau of Plant Genetic Resources, New Delhi 110 012, India

Abstract


Multiplexing in real-time PCR offers advantages over singleplex real-time PCR by saving time and re-sources. SYBR® Green I-based duplex and triplex re-al-time PCR assays targeting event-specific sequences of three genetically modified (GM) maize events, namely Bt11, Bt176 and MON89034, and taxon-specific endogenous Adh1 gene were developed to sim-ultaneously identify multiple events. Duplex real-time PCR assay based on TaqMan® chemistry targeting Bt176 event-specific sequence and Adh1 was also op-timized for quantification purpose. Limit of detection of developed assays was up to 0.05% and limit of quantification of the reported TaqMan® based real-time PCR was up to 0.5%.

Keywords


Dyes, Genetically Modified Maize, Gm De-Tection And Quantification, Multiplex Real-Time PCR, Pri-Mers and Probes.



DOI: https://doi.org/10.18520/cs%2Fv110%2Fi8%2F1446-1451