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dc.contributor.authorThibault Guinoiseauen_US
dc.contributor.authorAlain Moreauen_US
dc.contributor.authorGuillaume Hohnadelen_US
dc.contributor.authorNicole Ngo-Giang-Huongen_US
dc.contributor.authorCeline Brularden_US
dc.contributor.authorPatrick Vourc'Hen_US
dc.contributor.authorAlain Goudeauen_US
dc.contributor.authorCatherine Gaudy-Graffinen_US
dc.date.accessioned2018-09-05T03:27:28Z-
dc.date.available2018-09-05T03:27:28Z-
dc.date.issued2017-03-01en_US
dc.identifier.issn19326203en_US
dc.identifier.other2-s2.0-85016591258en_US
dc.identifier.other10.1371/journal.pone.0174852en_US
dc.identifier.urihttps://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=85016591258&origin=inwarden_US
dc.identifier.urihttp://cmuir.cmu.ac.th/jspui/handle/6653943832/56551-
dc.description.abstract© 2017 Guinoiseau et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Hepatitis C virus (HCV) evolves rapidly in a single host and circulates as a quasispecies wich is a complex mixture of genetically distinct virus's but closely related namely variants. To identify intra-individual diversity and investigate their functional properties in vitro, it is necessary to define their quasispecies composition and isolate the HCV variants. This is possible using single genome amplification (SGA). This technique, based on serially diluted cDNA to amplify a single cDNA molecule (clonal amplicon), has already been used to determine individual HCV diversity. In these studies, positive PCR reactions from SGA were directly sequenced using Sanger technology. The detection of non-clonal amplicons is necessary for excluding them to facilitate further functional analysis. Here, we compared Next Generation Sequencing (NGS) with De Novo assembly and Sanger sequencing for their ability to distinguish clonal and non-clonal amplicons after SGA on one plasma specimen. All amplicons (n = 42) classified as clonal by NGS were also classified as clonal by Sanger sequencing. No double peaks were seen on electropherograms for non-clonal amplicons with position-specific nucleotide variation below 15% by NGS. Altogether, NGS circumvented many of the difficulties encountered when using Sanger sequencing after SGA and is an appropriate tool to reliability select clonal amplicons for further functional studies.en_US
dc.subjectAgricultural and Biological Sciencesen_US
dc.subjectBiochemistry, Genetics and Molecular Biologyen_US
dc.titleDeep sequencing is an appropriate tool for the selection of unique Hepatitis C virus (HCV) variants after single genomic amplificationen_US
dc.typeJournalen_US
article.title.sourcetitlePLoS ONEen_US
article.volume12en_US
article.stream.affiliationsUniversite Francois-Rabelais Toursen_US
article.stream.affiliationsChiang Mai Universityen_US
Appears in Collections:CMUL: Journal Articles

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