Detection of rare mutations, copy number variation, and DNA methylation in the same template DNA molecules

Author:

Wang Yuxuan,Douville Christopher,Cohen Joshua D.,Mattox Austin,Curtis Sam,Silliman Natalie,Popoli Maria,Ptak Janine,Dobbyn Lisa,Nehme Nadine,Dudley Jonathan C.,Summers Mahmoud,Zhang Ming,Bettegowda Chetan,Papadopoulos Nickolas,Kinzler Kenneth W.,Vogelstein Bert

Abstract

ABSTRACTThe analysis of cell-free DNA (cfDNA) from plasma offers great promise for the earlier detection of cancer. At present, changes in DNA sequence, methylation, or copy number are the most sensitive ways to detect the presence of cancer. To further increase the sensitivity of such assays with limited amounts of sample, it would be useful to be able to evaluate the same template molecules for all these changes. Here we report an approach, called MethylSaferSeqS, that achieves this goal, and can be applied to any standard library preparation method suitable for massively parallel sequencing. The innovative step was to copy both strands of each DNA-barcoded molecule with a primer that allows the subsequent separation of the original strands (retaining their 5-methylcytosine residues) from the copied strands (in which the 5-methylcytosine residues are replaced with unmodified cytosine residues). The epigenetic and genetic alterations present in the DNA molecules can then be obtained from the original and copied strands, respectively. We applied this approach to plasma from 265 individuals, including 198 with cancers of the pancreas, ovary, lung and colon, and found the expected patterns of mutations, copy number alterations, and methylation. Furthermore, we could determine which original template DNA molecules were methylated and/or mutated. MethylSaferSeqS should be useful for addressing a variety of questions relating genetics and epigenetics in the future.

Publisher

Cold Spring Harbor Laboratory

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