2002
DOI: 10.1093/nar/gnf052
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High-throughput genotyping of single nucleotide polymorphisms using new biplex invader technology

Abstract: The feasibility of large-scale genome-wide association studies of complex human disorders depends on the availability of accurate and efficient genotyping methods for single nucleotide polymorphisms (SNPs). We describe a new platform of the invader assay, a biplex assay, where both alleles are interrogated in a single reaction tube. The assay was evaluated on over 50 different SNPs, with over 20 SNPs genotyped in study cohorts of over 1500 individuals. We assessed the usefulness of the new platform in high-thr… Show more

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Cited by 77 publications
(66 citation statements)
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“…As a quality standard, we randomly included six positive (two homozygous wild-type allele carriers, two heterozygous and two homozygous risk allele carriers) and two negative (all components excluding DNA) sequenced controls in each TaqMan reader plate. Because all controls were correctly identified, we assumed that the genotyping error rate of this method did not exceed 0.3% [23].…”
Section: Methodsmentioning
confidence: 99%
“…As a quality standard, we randomly included six positive (two homozygous wild-type allele carriers, two heterozygous and two homozygous risk allele carriers) and two negative (all components excluding DNA) sequenced controls in each TaqMan reader plate. Because all controls were correctly identified, we assumed that the genotyping error rate of this method did not exceed 0.3% [23].…”
Section: Methodsmentioning
confidence: 99%
“…All SNPs were genotyped using the biplex Invader assay, as previously described [38]. SNPs were genotyped on a set of 80 samples representing 10 independent three-generation CEPH families from Utah.…”
Section: Genotyping Of Single Nucleotide Polymorphismsmentioning
confidence: 99%
“…In addition, we included SNPs in and around the other apolipoprotein genes that were reported previously in association studies: SNPs 34, 35, and 36 are nonsynonymous changes in APOA4; SNPs 38 (APOC3 −482), 39 (APOC3 −455), and 41 (SstI) are located in APOC3; and SNP 43 (XmnI polymorphism) is located in APOA1 (see Table 1). All SNPs were genotyped using the biplex Invader assay, as previously described [38]. SNPs were genotyped on a set of 80 samples representing 10 independent three-generation CEPH families from Utah.…”
mentioning
confidence: 99%
“…As a quality standard, we randomly included six positive (2×A/A, 2×A/G, 2×G/G) and two negative (all components excluding DNA) sequenced controls in each TaqMan reader plate. Because all controls were correctly identified, we assumed that the genotyping error rate of this method did not exceed 0.3%, as demonstrated previously in a study designed to validate this method [17].…”
Section: Methodsmentioning
confidence: 99%