
pmid: 21637197
This protocol describes a new and rapid isothermal reaction process designed to amplify and detect a specific DNA sequence in purified DNA extracted from cultured cells. The protocol uses a DNA nanomachine that comprises two molecular switches that function in concert to isothermally amplify and detect a DNA target. First, a molecular beacon detection switch is 'activated' only if a DNA target sequence is present. A DNA primer and DNA polymerase are used to lock the beacon in an activated conformation. Second, an amplification and signal-transduction switch is initiated following successful activation. A nicking endonuclease and the DNA polymerase are used to replicate the DNA target. Both switches operate simultaneously at 40 °C in a single reaction to rapidly generate multiple copies of the DNA target in a cyclic polymerization reaction. This protocol enables femtomole amounts of a DNA target to be reproducibly amplified and detected in <40 min. We demonstrate the successful use of this protocol in assays containing synthetic DNA components and purified DNA extracted from biological samples.
1300 Biochemistry, Genetic analysis, Genetics and Molecular Biology, 612, DNA, Sequence Analysis, DNA, Biochemistry, Actins, Fluorescence, 1300 Biochemistry, Genetics and Molecular Biology, Nucleic Acid Amplification Techniques
1300 Biochemistry, Genetic analysis, Genetics and Molecular Biology, 612, DNA, Sequence Analysis, DNA, Biochemistry, Actins, Fluorescence, 1300 Biochemistry, Genetics and Molecular Biology, Nucleic Acid Amplification Techniques
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