Isolation and next generation sequencing of archival formalin-fixed DNA

J Anat. 2020 Sep;237(3):587-600. doi: 10.1111/joa.13209. Epub 2020 May 19.

Abstract

DNA from archived organs is presumed unsuitable for genomic studies because of excessive formalin-fixation. As next generation sequencing (NGS) requires short DNA fragments, and Uracil-N-glycosylase (UNG) can be used to overcome deamination, there has been renewed interest in the possibility of genomic studies using these collections. We describe a novel method of DNA extraction capable of providing PCR amplicons of at least 400 bp length from such excessively formalin-fixed human tissues. When compared with a leading commercial formalin-fixed DNA extraction kit, our method produced greater yields of DNA and reduced sequence variations. Analysis of PCR products using bacterial sub-cloning and Sanger sequencing from UNG-treated DNA unexpectedly revealed increased sequence variations, compared with untreated samples. Finally, whole exome NGS was performed on a myocardial sample fixed in formalin for 2 years and compared with lymphocyte-derived DNA (as a gold standard) from the same patient. Despite the reduction in the number and quality of reads in the formalin-fixed DNA, we were able to show that bioinformatic processing by joint calling and variant quality score recalibration (VQSR) increased the sensitivity four-fold to 56% and doubled specificity to 68% when compared with a standard hard-filtering approach. Thus, high-quality DNA can be extracted from excessively formalin-fixed tissues and bioinformatic processing can optimise sensitivity and specificity of results. Sequencing of several sub-cloned amplicons is an important methodological step in assessing DNA quality.

Keywords: Chelex 100; Uracil-N-glycosylase; archival DNA; formalin; next generation sequencing.

Publication types

  • Research Support, Non-U.S. Gov't

MeSH terms

  • DNA / isolation & purification*
  • Formaldehyde
  • High-Throughput Nucleotide Sequencing / methods*
  • Humans
  • Tissue Fixation*

Substances

  • Formaldehyde
  • DNA