PAP: Detection of ultra rare mutations depends on P* oligonucleotides: ?Sleeping Beauties? awakened by the kiss of pyrophosphorolysis

Liu, Qiang; Sommer, Steve S.

doi:10.1002/humu.20036

Cited by 34 publications

(35 citation statements)

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“…A method with high sensitivity is required in which the rare variant allele will not be overwhelmed by the large proportion of wild-type alleles. Numerous techniques have been developed to enhance the detection of the rare allele signal (19 ).…”

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confidence: 99%

Sensitive Detection of KIT D816V in Patients with Mastocytosis

et al. 2006

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Background: The 2447 A>T pathogenic variation at codon 816 of exon 17 (D816V) in the KIT gene, occurring in systemic mastocytosis (SM), leads to constitutive activation of tyrosine kinase activity and confers resistance to the tyrosine kinase inhibitor imatinib mesylate. Thus detection of this variation in SM patients is important for determining treatment strategy, but because the population of malignant cells carrying this variation is often small relative to the normal cell population, standard molecular detection methods can be unsuccessful. Methods: We developed 2 methods for detection of KIT D816V in SM patients. The first uses enriched sequencing of mutant alleles (ESMA) after BsmAI restriction enzyme digestion, and the second uses an allele-specific competitive blocker PCR (ACB-PCR) assay. We used these methods to assess 26 patients undergoing evaluation for SM, 13 of whom had SM meeting WHO classification criteria (before variation testing), and we compared the results with those obtained by direct sequencing. Results: The sensitivities of the ESMA and the ACB-PCR assays were 1% and 0.1%, respectively. According to the ACB-PCR assay results, 65% (17/26) of patients were positive for D816V. Of the 17 positive cases, only 23.5% (4/17) were detected by direct sequencing. ESMA detected 2 additional exon 17 pathogenic variations, D816Y and D816N, but detected only 12 (70.5%) of the

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confidence: 99%

Sensitive Detection of KIT D816V in Patients with Mastocytosis

et al. 2006

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“…By combining allele-specific PCR and serial coupling of pyrophosphorolysis, Liu Chiang Liu and Steve Sommer (City of Hope/Beckman Research Institute, Duarte, CA) succeeded in improving the specificity of primer extension and reported detection of one mutant SNP allele in the presence of up to 1 Â 10 9 copies of wild-type sequence in a lambda phage model system [Liu and Sommer, 2004].…”

Section: Sensitive Quantitative Mutation Detection and Snp Genotypingmentioning

confidence: 99%

Approaches for analyzing human mutations and nucleotide sequence variation: A report from the Seventh International Mutation Detection meeting, 2003

Syvänen

Taylor

2004

Hum. Mutat.

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The Seventh International Symposium on Mutations in the Human Genome, Mutation Detection 2003, was held during 2-6 July 2003 in Palm Cove near Cairns, Australia. The meeting was organized under the auspices of the Human Genome Organisation (HUGO) as a satellite meeting of the International World Congress of Genetics, held in Melbourne the following week. Meeting participants reported on advances in mutation detection technologies, including advances in high-throughput detection systems for SNP genotyping applicable to the international haplotype mapping project (HapMap); and bioinformatics tools, including databases for handling and processing growing amounts of genome variation data. This meeting report summarizes the presentations and cites related articles from the special issue of Human Mutation (Volume 23#5, May 2004; available online at www.wiley.com/humanmutation).

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“…Pyrophosphorolysis activated polymerization (PAP) was a technique originally developed to enhance the specificity of allele-specific PCR for detection of known mutants in the presence of an excess of the wild type allele (Liu and Sommer, 2004). Pyrophosphorolysis is the removal of the 3 nucleotide by DNA polymerase in the presence of pyrophosphate (PPi).…”

Section: Introductionmentioning

confidence: 99%

“…If the primer has fully annealed the DNA polymerase can remove the dideoxynucleotide by pyrophosphorolysis and extension can begin. As a result of the specific annealing which is required before extension, any nucleotide mismatch (within the first 15 nucleotides of the 3 prime end of the primer) between the primer and target will prevent the extension reaction from beginning (Liu and Sommer, 2004). If this technology could be applied to assaying the small proportion of cff DNA in the presence of the great excess of cfm DNA, then PAP could be a viable technology for NIPD.…”

Section: Introductionmentioning

confidence: 99%

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2008

Prenatal Diagnosis

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The discovery of cell-free fetal (cff) DNA and RNA in the maternal circulation has driven developments in noninvasive prenatal diagnosis (NIPD) for the past decade. Detection of paternally derived alleles in cff DNA is becoming well established. Now much interest is focussing on NIPD of fetal chromosomal abnormalities, such as trisomy 21, which is a considerable challenge because this demands accurate quantitative measurements of the amounts of specific cff DNA or cff RNA sequences in maternal blood samples. Emerging strategies for distinguishing and quantifying the fetal nucleic acids in the maternal circulation promise continued development of the field, and pose a number of unanswered questions.

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PAP: Detection of ultra rare mutations depends on P* oligonucleotides: ?Sleeping Beauties? awakened by the kiss of pyrophosphorolysis

Cited by 34 publications

References 59 publications

Sensitive Detection of KIT D816V in Patients with Mastocytosis

Sensitive Detection of KIT D816V in Patients with Mastocytosis

Approaches for analyzing human mutations and nucleotide sequence variation: A report from the Seventh International Mutation Detection meeting, 2003

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