Literature DB >> 26990372

A new virus discovered by immunocapture of double-stranded RNA, a rapid method for virus enrichment in metagenomic studies.

Arnaud G Blouin1,2, Howard A Ross2, Jody Hobson-Peters3, Caitlin A O'Brien3, Ben Warren1, Robin MacDiarmid1,2.   

Abstract

Next-generation sequencing technologies enable the rapid identification of viral infection of diseased organisms. However, despite a consistent decrease in sequencing costs, it is difficult to justify their use in large-scale surveys without a virus sequence enrichment technique. As the majority of plant viruses have an RNA genome, a common approach is to extract the double-stranded RNA (dsRNA) replicative form, to enrich the replicating virus genetic material over the host background. The traditional dsRNA extraction is time-consuming and labour-intensive. We present an alternative method to enrich dsRNA from plant extracts using anti-dsRNA monoclonal antibodies in a pull-down assay. The extracted dsRNA can be amplified by reverse transcriptase-polymerase chain reaction and sequenced by next-generation sequencing. In our study, we have selected three distinct plant hosts: Māori potato (Solanum tuberosum), rengarenga (Arthropodium cirratum) and broadleaved dock (Rumex obtusifolius) representing a cultivated crop, a New Zealand-native ornamental plant and a weed, respectively. Of the sequence data obtained, 31-74% of the reads were of viral origin, and we identified five viruses including Potato virus Y and Potato virus S in potato; Turnip mosaic virus in rengarenga (a new host record); and in the dock sample Cherry leaf roll virus and a novel virus belonging to the genus Macluravirus. We believe that this new assay represents a significant opportunity to upscale virus ecology studies from environmental, primary industry and/or medical samples.
© 2016 The Authors. Molecular Ecology Resources Published by John Wiley & Sons Ltd.

Entities:  

Keywords:  NGS; antibodies; dsRNA; metagenomics; plant virus

Mesh:

Substances:

Year:  2016        PMID: 26990372     DOI: 10.1111/1755-0998.12525

Source DB:  PubMed          Journal:  Mol Ecol Resour        ISSN: 1755-098X            Impact factor:   7.090


  15 in total

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4.  High-Throughput Sequencing and the Viromic Study of Grapevine Leaves: From the Detection of Grapevine-Infecting Viruses to the Description of a New Environmental Tymovirales Member.

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Journal:  Front Microbiol       Date:  2018-08-29       Impact factor: 5.640

5.  Comparison of Serological and Molecular Methods With High-Throughput Sequencing for the Detection and Quantification of Grapevine Fanleaf Virus in Vineyard Samples.

Authors:  Emmanuelle Vigne; Shahinez Garcia; Véronique Komar; Olivier Lemaire; Jean-Michel Hily
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6.  Immunocapture of virions with virus-specific antibodies prior to high-throughput sequencing effectively enriches for virus-specific sequences.

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7.  dsRNA-Seq: Identification of Viral Infection by Purifying and Sequencing dsRNA.

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8.  Updating the Quarantine Status of Prunus Infecting Viruses in Australia.

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Review 9.  Illuminating an Ecological Blackbox: Using High Throughput Sequencing to Characterize the Plant Virome Across Scales.

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Review 10.  Next-Generation Sequencing and Genome Editing in Plant Virology.

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Journal:  Front Microbiol       Date:  2016-08-26       Impact factor: 5.640

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