Evaluation of false positive and false negative errors in targeted next generation sequencing

Author:

Moon YoungbeenORCID,Kim Young-Ho,Kim Jong-Kwang,Hong Chung HwanORCID,Kang Eun-Kyung,Choi Hye Won,Lee Dong-eun,Kim Tae-Min,Heo Seong Gu,Han Namshik,Hong Kyeong-ManORCID

Abstract

AbstractBackgroundAlthough next generation sequencing (NGS) has been adopted as an essential diagnostic tool in various diseases, NGS errors have been the most serious problem in clinical implementation. Especially in cancers, low level mutations have not been easy to analyze, due to the contaminating normal cells and tumor heterozygosity.ResultsIn targeted NGS (T-NGS) analyses for reference-standard samples containing mixtures of homozygote H. mole DNA with blood genomic DNA at various ratios from four certified NGS service providers, large differences in the lower detection limit of variants (16.3 times, 1.51∼24.66%) and the false positive (FP) error rate (4280 times, 5.814 x 10−4∼1.359 x 10−7) were found. Employment of the commercially available Dragen system for bioinformatic analyses reduced FP errors in the results from companies BB and CC, but the errors originating from the NGS raw data persisted. Bioinformatic conditional adjustment to increase sensitivity (less than 2 times) led to a much higher FP error rate (610∼8200 times). In addition, problems such as biased preferential reference base calls during bioinformatic analysis and high-rate FN errors in HLA regions were found in the NGS analysis.ConclusionT-NGS results from certified NGS service providers can be quite various in their sensitivity and FP error rate, suggesting the necessity of further quality controls for clinical implementation of T-NGS. The present study also suggests that mixtures of homozygote and heterozygote DNAs can be easily employed as excellent reference-standard materials for quality control of T-NGS.

Publisher

Cold Spring Harbor Laboratory

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