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Rapid and reliable protocol for direct sequencing of material amplified by the polymerase chain reaction.
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1990
Year
EngineeringDna AnalysisMolecular BiologyNucleic Acid Amplification TestPcr ProductsGenomicsReal-time Polymerase Chain ReactionPolymerase Chain ReactionDirect SequencingReliable ProtocolDna SequencingMolecular Biological MethodDna ReplicationSequencingNext-generation SequencingBiotechnologySynthetic BiologyGenetic EngineeringNucleic Acid AmplificationMicrobiologyMedicineGenome Editing
A simple and reliable method is described for direct sequencing of material generated by the polymerase chain reaction. The protocol is based on the purification of the amplified double-stranded product by polyethylene glycol precipitation, annealing of primer with template by a "snap-cooling" procedure and sequencing by the dideoxy chain termination method with the use of Klenow fragment or Taq polymerase. The limit of the size of PCR products that can be sequenced is also discussed.