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Literature DB >> 12727909

DNA analysis by fluorescence quenching detection.

Abstract

The analysis of human genetic variations such as single nucleotide polymorphisms (SNPs) has great applications in genome-wide association studies of complex genetic traits. We have developed an SNP genotyping method based on the primer extension assay with fluorescence quenching as the detection. The template-directed dye-terminator incorporation with fluorescence quenching detection (FQ-TDI) assay is based on the observation that the intensity of fluorescent dye R110- and R6G-labeled acycloterminators is universally quenched once they are incorporated onto a DNA oligonucleotide primer. By comparing the rate of fluorescence quenching of the two allelic dyes in real time, we have extended this method for allele frequency estimation of SNPs in pooled DNA samples. The kinetic FQ-TDI assay is highly accurate and reproducible both in genotyping and in allele frequency estimation. Allele frequencies estimated by the kinetic FQ-TDI assay correlated well with known allele frequencies, with an r(2) value of 0.993. Applying this strategy to large-scale studies will greatly reduce the time and cost for genotyping hundreds and thousands of SNP markers between affected and control populations.

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Year: 2003 PMID： 12727909 PMCID： PMC430929 DOI： 10.1101/gr.987803

Source DB: PubMed Journal: Genome Res ISSN： 1088-9051 Impact factor: 9.043

17 in total

1. Prospects for whole-genome linkage disequilibrium mapping of common disease genes.

Authors: L Kruglyak
Journal: Nat Genet Date: 1999-06 Impact factor: 38.330

2. High-throughput SNP allele-frequency determination in pooled DNA samples by kinetic PCR.

Authors: S Germer; M J Holland; R Higuchi
Journal: Genome Res Date: 2000-02 Impact factor: 9.043

3. Determination of SNP allele frequencies in pooled DNAs by primer extension genotyping and denaturing high-performance liquid chromatography.

Authors: M Giordano; M Mellai; B Hoogendoorn; P Momigliano-Richiardi
Journal: J Biochem Biophys Methods Date: 2001-01-30

4. High-throughput SNP detection by using DNA pooling and denaturing high performance liquid chromatography (DHPLC).

Authors: J K Wolford; D Blunt; C Ballecer; M Prochazka
Journal: Hum Genet Date: 2000-11 Impact factor: 4.132

5. Effect of primary and secondary structure of oligodeoxyribonucleotides on the fluorescent properties of conjugated dyes.

Authors: Irina Nazarenko; Rick Pires; Brian Lowe; Mohamad Obaidy; Ayoub Rashtchian
Journal: Nucleic Acids Res Date: 2002-05-01 Impact factor: 16.971

6. Quantitative detection of single nucleotide polymorphisms for a pooled sample by a bioluminometric assay coupled with modified primer extension reactions (BAMPER).

Authors: G Zhou; M Kamahori; K Okano; G Chuan; K Harada; H Kambara
Journal: Nucleic Acids Res Date: 2001-10-01 Impact factor: 16.971

7. Universal SNP genotyping assay with fluorescence polarization detection.

Authors: T M Hsu; X Chen; S Duan; R D Miller; P Y Kwok
Journal: Biotechniques Date: 2001-09 Impact factor: 1.993

8. Estimation of single nucleotide polymorphism allele frequency in DNA pools by using Pyrosequencing.

Authors: Jonathan D Gruber; Peter B Colligan; Johanna K Wolford
Journal: Hum Genet Date: 2002-04-09 Impact factor: 4.132

9. Primer design for PCR and sequencing in high-throughput analysis of SNPs.

Authors: Ellen F Vieux; Pui-Yan Kwok; Raymond D Miller
Journal: Biotechniques Date: 2002-06 Impact factor: 1.993

10. Fluorescence-quenching phenomenon by photoinduced electron transfer between a fluorescent dye and a nucleotide base.

Authors: M Torimura; S Kurata; K Yamada; T Yokomaku; Y Kamagata; T Kanagawa; R Kurane
Journal: Anal Sci Date: 2001-01 Impact factor: 2.081

8 in total

1. Real-time closed tube single nucleotide polymorphism (SNP) quantification in pooled samples by quencher extension (QEXT).

Authors: Knut Rudi; Askild L Holck
Journal: Nucleic Acids Res Date: 2003-10-01 Impact factor: 16.971

DNA analysis by fluorescence quenching detection.

1. Prospects for whole-genome linkage disequilibrium mapping of common disease genes.

2. High-throughput SNP allele-frequency determination in pooled DNA samples by kinetic PCR.

3. Determination of SNP allele frequencies in pooled DNAs by primer extension genotyping and denaturing high-performance liquid chromatography.

4. High-throughput SNP detection by using DNA pooling and denaturing high performance liquid chromatography (DHPLC).

5. Effect of primary and secondary structure of oligodeoxyribonucleotides on the fluorescent properties of conjugated dyes.

6. Quantitative detection of single nucleotide polymorphisms for a pooled sample by a bioluminometric assay coupled with modified primer extension reactions (BAMPER).

7. Universal SNP genotyping assay with fluorescence polarization detection.

8. Estimation of single nucleotide polymorphism allele frequency in DNA pools by using Pyrosequencing.

9. Primer design for PCR and sequencing in high-throughput analysis of SNPs.

10. Fluorescence-quenching phenomenon by photoinduced electron transfer between a fluorescent dye and a nucleotide base.

1. Real-time closed tube single nucleotide polymorphism (SNP) quantification in pooled samples by quencher extension (QEXT).

2. A single molecular beacon probe is sufficient for the analysis of multiple nucleic acid sequences.

3. Rapid genotyping using pyrene-perylene locked nucleic acid complexes.

4. Rapid fixation of non-native alleles revealed by genome-wide SNP analysis of hybrid tiger salamanders.

5. Role of excess inorganic pyrophosphate in primer-extension genotyping assays.

6. Application of pooled genotyping to scan candidate regions for association with HDL cholesterol levels.

7. Multiplex SNP typing by bioluminometric assay coupled with terminator incorporation (BATI).

8. Development and Evaluation of an Enterovirus D68 Real-Time Reverse Transcriptase PCR Assay.