SiNVICT: ultra-sensitive detection of single nucleotide variants and indels in circulating tumour DNA

被引:43
|
作者
Kockan, Can [1 ,2 ]
Hach, Faraz [1 ,3 ]
Sarrafi, Iman [1 ]
Bell, Robert H. [3 ]
McConeghy, Brian [3 ]
Beja, Kevin [3 ]
Haegert, Anne [3 ]
Wyatt, Alexander W. [3 ,4 ]
Volik, Stanislav V. [3 ]
Chi, Kim N. [4 ]
Collins, Colin C. [3 ,4 ]
Sahinalp, Cenk [1 ,4 ,5 ]
机构
[1] Simon Fraser Univ, Sch Comp Sci, Burnaby, BC V5A 1S6, Canada
[2] Simon Fraser Univ, MADD Gen Grad Program, Burnaby, BC V5A 1S6, Canada
[3] Vancouver Prostate Ctr, Vancouver, BC V6H 3Z6, Canada
[4] Univ British Columbia, Dept Urol Sci, Vancouver, BC V6T 1Z4, Canada
[5] Indiana Univ, Sch Informat & Comp, Bloomington, IN 47405 USA
基金
加拿大自然科学与工程研究理事会;
关键词
CANCER; BIOMARKERS;
D O I
10.1093/bioinformatics/btw536
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Motivation: Successful development and application of precision oncology approaches require robust elucidation of the genomic landscape of a patient's cancer and, ideally, the ability to monitor therapy-induced genomic changes in the tumour in an inexpensive and minimally invasive manner. Thanks to recent advances in sequencing technologies, 'liquid biopsy', the sampling of patient's bodily fluids such as blood and urine, is considered as one of the most promising approaches to achieve this goal. In many cancer patients, and especially those with advanced metastatic disease, deep sequencing of circulating cell free DNA (cfDNA) obtained from patient's blood yields a mixture of reads originating from the normal DNA and from multiple tumour subclones-called circulating tumour DNA or ctDNA. The ctDNA/cfDNA ratio as well as the proportion of ctDNA originating from specific tumour subclones depend on multiple factors, making comprehensive detection of mutations difficult, especially at early stages of cancer. Furthermore, sensitive and accurate detection of single nucleotide variants (SNVs) and indels from cfDNA is constrained by several factors such as the sequencing errors and PCR artifacts, and mapping errors related to repeat regions within the genome. In this article, we introduce SiNVICT, a computational method that increases the sensitivity and specificity of SNV and indel detection at very low variant allele frequencies. SiNVICT has the capability to handle multiple sequencing platforms with different error properties; it minimizes false positives resulting from mapping errors and other technology specific artifacts including strand bias and low base quality at read ends. SiNVICT also has the capability to perform time-series analysis, where samples from a patient sequenced at multiple time points are jointly examined to report locations of interest where there is a possibility that certain clones were wiped out by some treatment while some subclones gained selective advantage. Results: We tested SiNVICT on simulated data as well as prostate cancer cell lines and cfDNA obtained from castration-resistant prostate cancer patients. On both simulated and biological data, SiNVICT was able to detect SNVs and indels with variant allele percentages as low as 0.5%. The lowest amounts of total DNA used for the biological data where SNVs and indels could be detected with very high sensitivity were 2.5 ng on the Ion Torrent platform and 10 ng on Illumina. With increased sequencing and mapping accuracy, SiNVICT might be utilized in clinical settings, making it possible to track the progress of point mutations and indels that are associated with resistance to cancer therapies and provide patients personalized treatment. We also compared SiNVICT with other popular SNV callers such as MuTect, VarScan2 and Freebayes. Our results show that SiNVICT performs better than these tools in most cases and allows further data exploration such as time-series analysis on cfDNA sequencing data.
引用
收藏
页码:26 / 34
页数:9
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