Nucleic Acids Research, Vol 25, Issue 17 3537-3542, Copyright © 1997 by Oxford University Press
SN Sheikh and P Lazarus
DNA covalently bound to an uncharged nylon membrane was used for
consecutive amplifications of several different genes by PCR. Successful
PCR amplifications were obtained for membrane-bound genomic and plasmid
DNA. Membrane-bound genomic DNA templates were re-used at least 15 times
for PCR with specific amplification of the desired gene each time. PCR
amplifications of specific sequences of p53, p16, CYP1A1, CYP2D6, GSTM1 and
GSTM3 were performed independently on the same strips of uncharged nylon
membrane containing genomic DNA. PCR products were subjected to restriction
fragment length polymorphism analysis, single-strand conformational
polymorphism analysis and/or dideoxy sequencing to confirm PCR-amplified
gene sequences. We found that PCR fragments obtained by amplification from
bound genomic DNA as template were identical in sequence to those of PCR
products obtained from free genomic DNA in solution. PCR was performed
using as little as 5 ng genomic or 4 fg plasmid DNA bound to membrane.
These results suggest that DNA covalently bound to membrane can be re-used
for sample- specific PCR amplifications, providing a potentially unlimited
source of DNA for PCR.
ARTICLES
Re-usable DNA template for the polymerase chain reaction
Department of Pathology and Laboratory Medicine, Temple University School of Medicine, 3400 North Broad Street, Philadelphia, PA 19140, USA.
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