Efficient and unbiased metagenomic recovery of RNA virus genomes from human plasma samples

Manso, Carmen F.; Bibby, David F.; Mbisa, Jean L.

doi:10.1038/s41598-017-02239-5

Cited by 32 publications

(28 citation statements)

References 71 publications

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“…Increasing the proportion of virus RNA for sequencing using cell culture is often difficult and may result in genetic variation that is not representative of the natural sample. Therefore, using total RNA extracted directly from natural host tissue is preferable in order to obtain evolutionarily relevant information on the virus genomes [11].…”

Section: Introductionmentioning

confidence: 99%

Assessing Genome-Wide Diversity in European Hantaviruses through Sequence Capture from Natural Host Samples

Hiltbrunner

Heckel

2020

Viruses

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Research on the ecology and evolution of viruses is often hampered by the limitation of sequence information to short parts of the genomes or single genomes derived from cultures. In this study, we use hybrid sequence capture enrichment in combination with high-throughput sequencing to provide efficient access to full genomes of European hantaviruses from rodent samples obtained in the field. We applied this methodology to Tula (TULV) and Puumala (PUUV) orthohantaviruses for which analyses from natural host samples are typically restricted to partial sequences of their tri-segmented RNA genome. We assembled a total of ten novel hantavirus genomes de novo with very high coverage (on average >99%) and sequencing depth (average >247×). A comparison with partial Sanger sequences indicated an accuracy of >99.9% for the assemblies. An analysis of two common vole (Microtus arvalis) samples infected with two TULV strains each allowed for the de novo assembly of all four TULV genomes. Combining the novel sequences with all available TULV and PUUV genomes revealed very similar patterns of sequence diversity along the genomes, except for remarkably higher diversity in the non-coding region of the S-segment in PUUV. The genomic distribution of polymorphisms in the coding sequence was similar between the species, but differed between the segments with the highest sequence divergence of 0.274 for the M-segment, 0.265 for the S-segment, and 0.248 for the L-segment (overall 0.258). Phylogenetic analyses showed the clustering of genome sequences consistent with their geographic distribution within each species. Genome-wide data yielded extremely high node support values, despite the impact of strong mutational saturation that is expected for hantavirus sequences obtained over large spatial distances. We conclude that genome sequencing based on capture enrichment protocols provides an efficient means for ecological and evolutionary investigations of hantaviruses at an unprecedented completeness and depth.

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Section: Introductionmentioning

confidence: 99%

Assessing Genome-Wide Diversity in European Hantaviruses through Sequence Capture from Natural Host Samples

Hiltbrunner

Heckel

2020

Viruses

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“…Viral discovery and identification from isolates and metagenomic samples present major challenges to bioinformatics in general. This is because viral genomes are prone to very high variability and deviation from reference genomes [42], continuous emergence of new viruses with no available references, high intrapopulation diversity, and the relative rareness of viral DNA fragments in metagenomic samples [43]. These challenges have largely been addressed through the following pipelines.…”

Section: Virus Discovery and Identification Toolsmentioning

confidence: 99%

Mosquito-Borne Viral Diseases: Control and Prevention in the Genomics Era

Fonseca¹,

Xavier²,

James³

et al. 2020

Vector-Borne Diseases - Recent Developments in Epidemiology and Control

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Mosquito-borne viral diseases are infections transmitted by the bite of infected mosquitoes. The burden of these diseases is highest in tropical and subtropical areas and they disproportionately affect the poorest populations. Since 2014, major outbreaks of dengue, chikungunya, yellow fever and Zika have afflicted populations and overwhelmed health systems in many countries. Distribution of mosquito-borne diseases is determined by complex demographic, environmental and social factors, causing diseases to emerge in countries where they were previously unknown. Coupling genomic diagnostics and epidemiology to innovative digital disease detection platforms raises the possibility of an open, global, digital pathogen surveillance system. Considering pathogen surveillance in mind, real-time sequencing, bioinformatics tools and the combination of genomic and epidemiological data from viral infections can give essential information for understanding the past and the future of an epidemic, making possible to establish an effective surveillance framework on tracking the spread of infections to other geographic regions.

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“…Improving this ratio is key to achieving a sufficient amount of viral reads to allow reliable detection and accurate identification of viruses in a sample ( Chan et al, 2014 ; Hall et al, 2014 ; Kohl et al, 2015 ; Lewandowska et al, 2015 ; Bukowska-Ośko et al, 2017 ). Selective depletion of the ribosomal RNA (rRNA) fraction followed by DNAse digestion resulted in a significant methodological improvement in the mNGS protocol for RNA viruses previously developed in our laboratory ( Manso et al, 2017 ). However, effective enrichment of viral DNA has proven to be more challenging due to the lack of differential motifs between human and viral DNA that allow depleting the former without affecting the number of copies of the latter in the sample.…”

Section: Introductionmentioning

confidence: 99%

Enhanced Detection of DNA Viruses in the Cerebrospinal Fluid of Encephalitis Patients Using Metagenomic Next-Generation Sequencing

et al. 2020

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The long and expanding list of viral pathogens associated with causing encephalitis confounds current diagnostic procedures, and in up to 50% of cases, the etiology remains undetermined. Sequence-agnostic metagenomic next-generation sequencing (mNGS) obviates the need to specify targets in advance and thus has great potential in encephalitis diagnostics. However, the low relative abundance of viral nucleic acids in clinical specimens poses a significant challenge. Our protocol employs two novel techniques to selectively remove human material at two stages, significantly increasing the representation of viral material. Our bioinformatic workflow using open source protein- and nucleotide sequence-matching software balances sensitivity and specificity in diagnosing and characterizing any DNA viruses present. A panel of 12 cerebrospinal fluid (CSFs) from encephalitis cases was retrospectively interrogated by mNGS, with concordant results in seven of nine samples with a definitive DNA virus diagnosis, and a different herpesvirus was identified in the other two. In two samples with an inconclusive diagnosis, DNA viruses were detected and in a virus-negative sample, no viruses were detected. This assay has the potential to detect DNA virus infections in cases of encephalitis of unknown etiology and to improve the current screening tests by identifying new and emerging agents.

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Efficient and unbiased metagenomic recovery of RNA virus genomes from human plasma samples

Cited by 32 publications

References 71 publications

Assessing Genome-Wide Diversity in European Hantaviruses through Sequence Capture from Natural Host Samples

Assessing Genome-Wide Diversity in European Hantaviruses through Sequence Capture from Natural Host Samples

Mosquito-Borne Viral Diseases: Control and Prevention in the Genomics Era

Enhanced Detection of DNA Viruses in the Cerebrospinal Fluid of Encephalitis Patients Using Metagenomic Next-Generation Sequencing

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