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Detection and measurement of PCR bias in quantitative methylation analysis of bisulphite-treated DNA
- Source :
- Nucleic Acids Research. 25:4422-4426
- Publication Year :
- 1997
- Publisher :
- Oxford University Press (OUP), 1997.
-
Abstract
- Methylation analysis of individual cytosines in genomic DNA can be determined quantitatively by bisulphite treatment and PCR amplification of the target DNA sequence, followed by restriction enzyme digestion or sequencing. Methylated and unmethylated molecules, however, have different sequences after bisulphite conversion. For some sequences this can result in bias during the PCR amplification leading to an inaccurate estimate of methylation. PCR bias is sequence dependent and often strand-specific. This study presents a simple method for detection and measurement of PCR bias for any set of primers, and investigates parameters for overcoming PCR bias.
- Subjects :
- Biology
Polymerase Chain Reaction
Sensitivity and Specificity
DNA sequencing
Cell Line
law.invention
Cytosine
Mice
chemistry.chemical_compound
law
Primer dimer
Genetics
Animals
Humans
Sulfites
Genes, Retinoblastoma
Polymerase chain reaction
DNA Primers
Base Composition
Multiple displacement amplification
DNA
DNA Methylation
Molecular biology
genomic DNA
5-Methylcytosine
chemistry
DNA methylation
Research Article
In silico PCR
Subjects
Details
- ISSN :
- 13624962 and 03051048
- Volume :
- 25
- Database :
- OpenAIRE
- Journal :
- Nucleic Acids Research
- Accession number :
- edsair.doi.dedup.....b244ed9035c1d5be8a2bd9a4c979a880
- Full Text :
- https://doi.org/10.1093/nar/25.21.4422