Abstract
Next-generation sequencing (NGS) studies are becoming routinely used for the detection of novel and clinically actionable DNA variants at a pangenomic scale. Such analyses are now used in the clinical practice to enable precision medicine. Formalin-fixed paraffin-embedded (FFPE) tissues are still one of the most abundant source of cancer clinical specimen, unfortunately this method of preparation is known to degrade DNA and therefore compromise subsequent analysis. Some studies have reported that variant detection can be performed on FFPE samples sequenced with NGS techniques, but few or none have done an in-depth coverage analysis and compared the influence of different state-of-the-art FFPE DNA extraction kits on the quality of the variant calling. Here, we generated 42 human whole-exome sequencing data sets from fresh-frozen (FF) and FFPE samples. These samples include normal and tumor tissues from two different organs (liver and colon), that we extracted with three different FFPE extraction kits (QIAamp DNA FFPE Tissue kit and GeneRead DNA FFPE kit from Qiagen, Maxwell™ RSC DNA FFPE Kit from Promega). We determined the rate of concordance of called variants between matched FF and FFPE samples on all common variants (representing at least 86% of the total number of variants for SNVs). The concordance rate is very high between all matched FF / FFPE pairs, with equivalent values for the three kits we analyzed. On the other hand, when looking at the difference between the total number of variants in FF and FFPE, we find a significant variation for the three different FFPE DNA extraction kits. Coverage analysis shows that FFPE samples have less good indicators than FF samples, yet the coverage quality remains above accepted thresholds. We detect limited but statistically significant variations in coverage indicator values between the three FFPE extraction kits. Globally, the GeneRead and QIAamp kits have better variant calling and coverage indicators than the Maxwell kit on the samples used in this study, although this kit performs better on some indicators and has advantages in terms of practical usage. Taken together, our results confirm the potential of FFPE samples analysis for clinical genomic studies, but also indicate that the choice of a FFPE DNA extraction kit should be done with careful testing and analysis beforehand in order to maximize the accuracy of the results.
Highlights
Next-generation sequencing (NGS) approaches have proven to be a cost-effective and relevant method for the identification of novel and clinically actionable variants across many genes in a single test [1,2,3,4,5,6,7]
We find a significant difference for the DNA Integrity Number (DIN) values between the three extraction methods for the Formalin-fixed paraffin-embedded (FFPE) samples (Fig 1B, one-way anova, F-value = 19.7, df = 2, p-value = 1.03e-5)
We systematically analyzed coverage indicators and performed variant analysis between FF and FFPE samples, and we analyzed the influence of three different FFPE DNA extraction kits by comparing matched pairs of FF and FFPE samples
Summary
Next-generation sequencing (NGS) approaches have proven to be a cost-effective and relevant method for the identification of novel and clinically actionable variants across many genes in a single test [1,2,3,4,5,6,7]. Formaldehyde is known to induce oxidation and deamination reactions and the formation of cyclic bases derivatives. These chemical modifications have the potential to alter molecular testing through inhibition of enzymatic reparation of DNA or direct changes at single base or sequence levels. Crosslinks lead to DNA fragmentation that render sequencing and analysis even more complicated [11,12,13,14,15,16]
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