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Reliable and efficient direct sequencing of PCR-amplified double-stranded genomic DNA template.

作者信息

Jung M, Dritschilo A, Kasid U

机构信息

Department of Radiation Medicine, Georgetown University Medical Center, Washington, DC 20007.

出版信息

PCR Methods Appl. 1992 Feb;1(3):171-4. doi: 10.1101/gr.1.3.171.

Abstract

Modified PCR amplification and direct sequencing procedures for the double-stranded genomic DNA template are described. Advantages of the approach we describe are: background artifact bands previously observed using high-molecular-weight DNA as a template were eliminated by this protocol; no gel purification or subcloning of the PCR-amplified double-stranded fragment was required prior to direct sequencing; and sequences of 300 nucleotides can be easily read even after a single loading. The successful use of the modified dideoxynucleotide chain-termination method for direct sequencing of both strands demonstrates the efficiency of this technique for removing sequencing artifacts and for producing reliable sequence data.

摘要

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