Structural variation and fusion detection using targeted sequencing data from circulating cell free DNA

Alexander R Gawroński; Yen-Yi Lin; Brian McConeghy; Stephane LeBihan; Hossein Asghari; Can Koçkan; Baraa Orabi; Nabil Adra; Roberto Pili; Colin C Collins; S Cenk Sahinalp; Faraz Hach

doi:10.1093/nar/gkz067

Structural variation and fusion detection using targeted sequencing data from circulating cell free DNA

Nucleic Acids Res. 2019 Apr 23;47(7):e38. doi: 10.1093/nar/gkz067.

Authors

Alexander R Gawroński¹, Yen-Yi Lin^{2

3}, Brian McConeghy^{2

3}, Stephane LeBihan^{2

3}, Hossein Asghari^{1

3}, Can Koçkan⁴, Baraa Orabi^{1

3}, Nabil Adra⁵, Roberto Pili⁵, Colin C Collins^{2

3}, S Cenk Sahinalp⁴, Faraz Hach^{2

3}

Affiliations

¹ School of Computing Science, Simon Fraser University, Burnaby, British Columbia V5A 1S6, Canada.
² Department of Urologic Sciences, Faculty of Medicine, University of British Columbia, Vancouver, British Columbia V52 1M9, Canada.
³ Vancouver Prostate Centre, Vancouver, British Columbia V6H 3Z6, Canada.
⁴ Department of Computer Science, Indiana University, Bloomington 47405, USA.
⁵ School of Medicine, Indiana University, Indianapolis, 46202, USA.

Abstract

Motivation: Cancer is a complex disease that involves rapidly evolving cells, often forming multiple distinct clones. In order to effectively understand progression of a patient-specific tumor, one needs to comprehensively sample tumor DNA at multiple time points, ideally obtained through inexpensive and minimally invasive techniques. Current sequencing technologies make the 'liquid biopsy' possible, which involves sampling a patient's blood or urine and sequencing the circulating cell free DNA (cfDNA). A certain percentage of this DNA originates from the tumor, known as circulating tumor DNA (ctDNA). The ratio of ctDNA may be extremely low in the sample, and the ctDNA may originate from multiple tumors or clones. These factors present unique challenges for applying existing tools and workflows to the analysis of ctDNA, especially in the detection of structural variations which rely on sufficient read coverage to be detectable.

Results: Here we introduce SViCT , a structural variation (SV) detection tool designed to handle the challenges associated with cfDNA analysis. SViCT can detect breakpoints and sequences of various structural variations including deletions, insertions, inversions, duplications and translocations. SViCT extracts discordant read pairs, one-end anchors and soft-clipped/split reads, assembles them into contigs, and re-maps contig intervals to a reference genome using an efficient k-mer indexing approach. The intervals are then joined using a combination of graph and greedy algorithms to identify specific structural variant signatures. We assessed the performance of SViCT and compared it to state-of-the-art tools using simulated cfDNA datasets with properties matching those of real cfDNA samples. The positive predictive value and sensitivity of our tool was superior to all the tested tools and reasonable performance was maintained down to the lowest dilution of 0.01% tumor DNA in simulated datasets. Additionally, SViCT was able to detect all known SVs in two real cfDNA reference datasets (at 0.6-5% ctDNA) and predict a novel structural variant in a prostate cancer cohort.

Availability: SViCT is available at https://github.com/vpc-ccg/svict. Contact:faraz.hach@ubc.ca.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Algorithms*
Cell-Free Nucleic Acids / blood*
Cell-Free Nucleic Acids / genetics*
Circulating Tumor DNA / blood
Circulating Tumor DNA / genetics
DNA Mutational Analysis / methods*
Datasets as Topic
Humans
Male
Mutation*
Prostatic Neoplasms / genetics
Sensitivity and Specificity

Substances

Cell-Free Nucleic Acids
Circulating Tumor DNA

Grants and funding

R01 GM108348/GM/NIGMS NIH HHS/United States