BioTechniques (Dec 2006)

Rapid and quantitative method of allele-specific DNA methylation analysis

  • Hui-Lee Wong,
  • Hyang-Min Byun,
  • Jennifer M. Kwan,
  • Mihaela Campan,
  • Sue A. Ingles,
  • Peter W. Laird,
  • Allen S. Yang

DOI
https://doi.org/10.2144/000112305
Journal volume & issue
Vol. 41, no. 6
pp. 734 – 739

Abstract

Read online

Several biological phenomena depend on differential methylation of chromosomal strands. While understanding the role of these processes requires information on allele-specific methylation, the available methodologies are not quantitative or labor-intensive. We describe a novel, rapid method to quantitate allele-specific DNA methylation based on the combination of bisulfite PCR and Pyrosequencing™. In this method, DNA is first treated with sodium bisulfite, which converts cytosine but not 5-methylcytosine to uracil. Genes of interest are subsequently amplified using PCR. Allele-specific methylation can then be determined by pyrosequencing each allele individually using sequencing primers that incorporate single nucleotide polymorphisms (SNPs) that allow differentiation between the two parental alleles. This allele-specific methylation methodology can potentially afford quantitative analyses relevant to the regulation of X chromosome inactivation, allele-specific expression of genes in the immune system, repetitive elements, and genomic imprinting. As an illustration of our new method, we quantitated allele-specific methylation of the differentially methylated region of the H19 gene, which is imprinted. Although we could reliably determine allele-specific methylation with our technique, additional studies will be required to confirm the ability of our assay to measure loss of imprinting.