DNA methylation is an epigenetic process that plays a critical role in gene expression modulation and has been implicated in many diseases, particularly cancer. One method to study the variability in methylation patterns is whole-genome bisulfite sequencing (WGBS), which analyzes single base methylation through immunoprecipitations using antibody or methyl binding domain proteins. While WGBS enables the analysis of DNA methylation with single base resolutions, it degrades DNA, requires microgram amounts of input DNA and purification. Further it is cost prohibitive and cannot distinguish between some distinct epigenetic modifications. Another method is Methylated DNA immunoprecipitation followed by sequencing (MeDIP-seq) which enriches methylated DNA fragments using monoclonal antibodies. This method has decent resolution and can detect differentially methylated regions, but it is incapable of multiplexed analyses.
Researchers at the Biodesign Institute of Arizona State University have developed a novel method to perform multiplexed methylated DNA immunoprecipitation sequencing (Mx-MeDIP-Seq). Because every run of the Mx-MeDIP-Seq can contain up to 15 different samples, this technique can analyze massive numbers of DNA in a parallel manner with low DNA input amounts. With as little as 10 ng of input DNA a greater than 95% specificity can be achieved and with as little as 1 ng input DNA, a greater than 75% specificity can be achieved. To demonstrate the reliability of the multiplexed protocol, MeDIP was performed, individually, on the same samples as those for Mx-MeDIP-Seq, and showed similar results.
This novel technique provides a simpler, faster and more cost-effect method for DNA methylation analyses in a multiplexed format.
Potential Applications
Benefits and Advantages
For more information about the inventor(s) and their research, please see
Dr. LaBaer's Biodesign Institute webpage
Dr. Murugan’s Biodesign Institute webpage