Issue 4, 2009

Quadruple-allele chemiluminometric assay for simultaneous genotyping of two single-nucleotide polymorphisms

Abstract

We developed a rapid, simple, cost-effective and high sample-throughput method for the simultaneous detection of four alleles in single-nucleotide polymorphisms (SNPs). The method was applied to the simultaneous genotyping of two common SNPs within the TLR4 gene, the A896G and C1196T polymorphisms. The method consists of a single PCR of the region spanning the A896G and C1196T polymorphic sites, followed by a quadruple primer extension (PEXT) reaction in a single tube. A biotinylated nucleotide is incorporated in the extended primer. All four products are captured in streptavidin (SA)-coated microtiter wells and detected with a combination of four reporters, the photoprotein aequorin (AEQ) and the enzymes alkaline phosphatase (ALP), β-galactosidase (GAL) and horseradish peroxidase (HRP). For each SNP, 46 individuals were genotyped. The accuracy of this method was confirmed by sequencing. The proposed quadruple-allele chemiluminometric assay provides an accurate, simple, rapid, reproducible and cost-effective method for high sample-throughput genotyping of single-nucleotide polymorphisms.

Graphical abstract: Quadruple-allele chemiluminometric assay for simultaneous genotyping of two single-nucleotide polymorphisms

Article information

Article type
Paper
Submitted
20 Oct 2008
Accepted
16 Dec 2008
First published
14 Jan 2009

Analyst, 2009,134, 725-730

Quadruple-allele chemiluminometric assay for simultaneous genotyping of two single-nucleotide polymorphisms

D. S. Elenis, P. C. Ioannou and T. K. Christopoulos, Analyst, 2009, 134, 725 DOI: 10.1039/B818516F

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