Utility of cfDNA Fragmentation Patterns in Designing the Liquid Biopsy Profiling Panels to Improve Their Sensitivity

Maxim Ivanov; Polina Chernenko; Valery Breder; Konstantin Laktionov; Ekaterina Rozhavskaya; Sergey Musienko; Ancha Baranova; Vladislav Mileyko

doi:10.3389/fgene.2019.00194

Utility of cfDNA Fragmentation Patterns in Designing the Liquid Biopsy Profiling Panels to Improve Their Sensitivity

Front Genet. 2019 Mar 12:10:194. doi: 10.3389/fgene.2019.00194. eCollection 2019.

Authors

Affiliations

¹ Department of Biological and Medical Physics, Moscow Institute of Physics and Technology, Dolgoprudny, Russia.
² N.N. Blokhin Russian Cancer Research Center, Moscow, Russia.
³ Atlas Oncology Diagnostics, Ltd., Moscow, Russia.
⁴ Vavilov Institute of General Genetics, Moscow, Russia.
⁵ Research Centre for Medical Genetics, Moscow, Russia.
⁶ School of Systems Biology, George Mason University, Fairfax, VA, United States.

Abstract

Genotyping of cell-free DNA (cfDNA) in plasma samples has the potential to allow for a noninvasive assessment of tumor biology, avoiding the inherent shortcomings of tissue biopsy. Next generation sequencing (NGS), a leading technology for liquid biopsy analysis, continues to be hurdled with several major issues with cfDNA samples, including low cfDNA concentration and high fragmentation. In this study, by employing Ion Torrent PGM semiconductor technology, we performed a comparison between two multi-biomarker amplicon-based NGS panels characterized by a substantial difference in average amplicon length. In course of the analysis of the peripheral blood from 13 diagnostic non-small cell lung cancer patients, equivalence of two panels, in terms of overall diagnostic sensitivity and specificity was shown. A pairwise comparison of the allele frequencies for the same somatic variants obtained from the pairs of panel-specific amplicons, demonstrated an identical analytical sensitivity in range of 140 to 170 bp amplicons in size. Further regression analysis between amplicon length and its coverage, illustrated that NGS sequencing of plasma cfDNA equally tolerates amplicons with lengths in the range of 120 to 170 bp. To increase the sensitivity of mutation detection in cfDNA, we performed a computational analysis of the features associated with genome-wide nucleosome maps, evident from the data on the prevalence of cfDNA fragments of certain sizes and their fragmentation patterns. By leveraging the support vector machine-based machine learning approach, we showed that a combination of nucleosome map associated features with GC content, results in the increased accuracy of prediction of high inter-sample sequencing coverage variation (areas under the receiver operating curve: 0.75, 95% CI: 0.750-0.752 vs. 0.65, 95% CI: 0.63-0.67). Thus, nucleosome-guided fragmentation should be utilized as a guide to design amplicon-based NGS panels for the genotyping of cfDNA samples.

Keywords: DNA fragmentation; NGS; amplicon; cancer; cfDNA; liquid biopsy; nucleosome; primer design.