Simultaneous Determination of 7 N-Acetyltransferase-2 Sequence Variations by Allele-Specific Primer Extension Assay

doi:10.1373/clinchem.2005.063198

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Clinical Chemistry 0: clinchem.2005.063198v1, 2006; 10.1373/clinchem.2005.063198

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Received on November 3, 2005
Accepted on February 23, 2006

Molecular Diagnostics and Genetics

Simultaneous Determination of 7 N-Acetyltransferase-2 Sequence Variations by Allele-Specific Primer Extension Assay

Yusheng Zhu ¹, David W. Hein ², Mark A. Doll ³, Kristen K. Reynolds ¹, Ntei Abudu ¹, Roland Valdes Jr.⁴, Mark W. Linder ¹^*

¹ Department of Pathology and Laboratory Medicine, University of Louisville School of Medicine, Louisville, KY
² Department of Pharmacology and Toxicology, University of Louisville School of Medicine, Louisville, KY
³ Department of Pharmacology and Toxicology, University of Louisville School of Medicine, Louisville, KY
⁴ Department of Pathology and Laboratory, University of Louisville School of Medicine, Louisville, KY

^* To whom correspondence should be addressed. E-mail: mwlind01{at}gwise.louisville.edu.

Background: Genotyping of N-acetyltransferase-2 (NAT2) is usefulin predicting the risk for toxicity of NAT2 substrates. Currentmethods cannot detect the 7 most important single-nucleotidevariations in NAT2 simultaneously in 1 tube.

Methods: We developedan assay that uses allele-specific primer extension (ASPE) andmicrosphere hybridization for the simultaneous detection of7 single-nucleotide variations in NAT2. Using 12 samples previouslygenotyped by a TaqMan-based assay for method development andas positive controls, we amplified the genetic locus of NAT2comprising the single-nucleotide variations of interest by PCRand then performed ASPE with allele-specific primers and biotinylateddCTP followed by bead hybridization and streptavidin-R-phycoerythrinbinding. Genotypes were determined according to the allele-specificfluorescent signal ratios.

Results: The mean (SD) allelic ratiosfor homozygous common, heterozygous variant, and homozygousvariant NAT2 genotypes were 0.0394 (0.0113) (n = 80), 0.4372(0.0270) (n = 148), and 0.9331 (0.0127) (n = 325). The assayhad 100% (95% confidence interval, 99%-100%) within-run reproducibilityfor 12 samples repeated 6 times and 100% (98%-100%) between-runreproducibility for a 5-sample subset run on 6 different days.NAT2 genotypes of 30 blinded samples determined by this assaywere 100% (98%-100%) concordant with results obtained usingthe TaqMan method.

Conclusions: The developed assay can simultaneouslydetermine single-nucleotide variations in NAT2. The assay demonstratesno overlap in allele-specific signal ratios between homozygouscommon, heterozygous, and homozygous variant and shows agreementwith a reference method and reproducibility of genotype identification.

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