PCR candidate region mismatch scanning: adaptation to quantitative, high-throughput genotyping

doi:10.1093/nar/29.5.1114

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Nucleic Acids Research, 2001, Vol. 29, No. 5 1114-1124
© 2001 Oxford University Press

PCR candidate region mismatch scanning: adaptation to quantitative, high-throughput genotyping

Martin Beaulieu, Garry P. Larson, Louis Geller, Steven D. Flanagan¹ and Theodore G. Krontiris^*

Division of Molecular Medicine and ¹Division of Neurosciences, Beckman Research Institute, City of Hope National Medical Center, Duarte, CA 91010, USA

Linkage and association analyses were performed to identifyloci affecting disease susceptibility by scoring previouslycharacterized sequence variations such as microsatellites andsingle nucleotide polymorphisms. Lack of markers in regionsof interest, as well as difficulty in adapting various methodsto high-throughput settings, often limits the effectivenessof the analyses. We have adapted the Escherichia coli mismatchdetection system, employing the factors MutS, MutL and MutH,for use in PCR-based, automated, high-throughput genotypingand mutation detection of genomic DNA. Optimal sensitivity andsignal-to-noise ratios were obtained in a straightforward fashionbecause the detection reaction proved to be principally dependentupon monovalent cation concentration and MutL concentration.Quantitative relationships of the optimal values of these parameterswith length of the DNA test fragment were demonstrated, in supportof the translocation model for the mechanism of action of theseenzymes, rather than the molecular switch model. Thus, rapid,sequence-independent optimization was possible for each newgenomic target region. Other factors potentially limiting theflexibility of mismatch scanning, such as positioning of damrecognition sites within the target fragment, have also beeninvestigated. We developed several strategies, which can beeasily adapted to automation, for limiting the analysis to intersampleheteroduplexes. Thus, the principal barriers to the use of thismethodology, which we have designated PCR candidate region mismatchscanning, in cost-effective, high-throughput settings have beenremoved.

^* To whom correspondence should be addressed. Tel: +1 626 3598111; Fax: +1 626 301 8862; Email: tkrontir{at}coh.org

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