1. Two-fold differences are the detection limit for determining transgene copy numbers in plants by real-time PCR
- Author
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Bubner, B., Gase, K., and Baldwin, I.
- Subjects
Heterozygote ,DNA, Complementary ,DNA, Plant ,lcsh:Biotechnology ,Methodology Article ,Genetic Vectors ,Gene Amplification ,Gene Dosage ,Genetic Variation ,Plants ,Plants, Genetically Modified ,Polymerase Chain Reaction ,Computer Systems ,lcsh:TP248.13-248.65 ,Transgenes ,DNA Probes - Abstract
Background After transformation, plants that are homozygous and contain one copy of the transgene are typically selected for further study. If real-time PCR is to be used to determine copy number and zygosity, it must be able to distinguish hemizygous from homozygous and one-copy from two-copy plants. That is, it must be able to detect two-fold differences. Results When transgenic Nicotiana attenuata plants which had been previously determined by Southern analysis to contain one or two copies of the transgene, were analyzed by real-time PCR (2-ΔΔCt method), the method failed to confirm the results from the Southern analysis. In a second data set we analyzed offspring of a hemizygous one-copy plant, which were expected to segregate into three groups of offspring in a 1:2:1 ratio: no transgene, hemizygous, homozygous. Because it was not possible to distinguish homozygous from hemizygous plants with real-time PCR, we could not verify this segregation ratio. Conclusions Detection of two-fold differences by real-time PCR is essential if this procedure is to be used for the characterization of transgenic plants. However, given the high variability between replicates, a detection of two-fold differences is in many cases not possible; in such cases Southern analysis is the more reliable procedure.
- Published
- 2004