| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2091008 | Journal of Microbiological Methods | 2008 | 5 Pages |
Abstract
We developed and tested a method to produce DNA standards and controls for quantitative PCR by designing and performing partial hybridization of long oligonucleotides before double stranded DNA fragments were synthesized and subsequently amplified by conventional PCR. This approach does not require any natural DNA template. Applications include the production of standards, which cannot be easily produced from DNA extracted from bacteria or plants.
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Authors
Maude M. David, Amy R. Sapkota, Pascal Simonet, Timothy M. Vogel,