Enrichment post-library preparation enhances the sensitivity of high-throughput sequencing-based detection and characterization of viruses from complex samples

Adrian C. Paskey; Kenneth G. Frey; Gary Schroth; Stephen Gross; Theron Hamilton; Kimberly A. Bishop-Lilly

doi:10.1186/s12864-019-5543-2

BMC Genomics (Feb 2019)

Enrichment post-library preparation enhances the sensitivity of high-throughput sequencing-based detection and characterization of viruses from complex samples

Adrian C. Paskey,
Kenneth G. Frey,
Gary Schroth,
Stephen Gross,
Theron Hamilton,
Kimberly A. Bishop-Lilly

Affiliations

Adrian C. Paskey: Genomics and Bioinformatics Department, Biological Defense Research Directorate, Naval Medical Research Center – Frederick
Kenneth G. Frey: Genomics and Bioinformatics Department, Biological Defense Research Directorate, Naval Medical Research Center – Frederick
Gary Schroth: Illumina Inc.
Stephen Gross: Illumina Inc.
Theron Hamilton: Genomics and Bioinformatics Department, Biological Defense Research Directorate, Naval Medical Research Center – Frederick
Kimberly A. Bishop-Lilly: Genomics and Bioinformatics Department, Biological Defense Research Directorate, Naval Medical Research Center – Frederick

DOI: https://doi.org/10.1186/s12864-019-5543-2
Journal volume & issue: Vol. 20, no. 1
pp. 1 – 14

Abstract

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Abstract Background Sequencing-based detection and characterization of viruses in complex samples can suffer from lack of sensitivity due to a variety of factors including, but not limited to, low titer, small genome size, and contribution of host or environmental nucleic acids. Hybridization-based target enrichment is one potential method for increasing the sensitivity of viral detection via high-throughput sequencing. Results This study expands upon two previously developed panels of virus enrichment probes (for filoviruses and for respiratory viruses) to include other viruses of biodefense and/or biosurveillance concern to the U.S. Department of Defense and various international public health agencies. The newly expanded and combined panel is tested using carefully constructed synthetic metagenomic samples that contain clinically relevant amounts of viral genetic material. Target enrichment results in a dramatic increase in sensitivity for virus detection as compared to shotgun sequencing, yielding full, deeply covered viral genomes from materials with Ct values suggesting that amplicon sequencing would be likely to fail. Increased pooling to improve cost- and time-effectiveness does not negatively affect the ability to obtain full-length viral genomes, even in the case of co-infections, although as expected, it does decrease depth of coverage. Conclusions Hybridization-based target enrichment is an effective solution to obtain full-length viral genomes for samples from which virus detection would fail via unbiased, shotgun sequencing or even via amplicon sequencing. As the development and testing of probe sets for viral target enrichment expands and continues, the application of this technique, in conjunction with deeper pooling strategies, could make high-throughput sequencing more economical for routine use in biosurveillance, biodefense and outbreak investigations.

Published in BMC Genomics

ISSN: 1471-2164 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Technology: Chemical technology: Biotechnology; Science: Biology (General): Genetics
Website: http://bmcgenomics.biomedcentral.com

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Abstract

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