Characterization of a major V3 duplication in the NS5A region of genotype 1b HCV by quasispecies analysis in a French multicenter study

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ID Serval
serval:BIB_7F3A5A70D8E4
Type
Actes de conférence (partie): contribution originale à la littérature scientifique, publiée à l'occasion de conférences scientifiques, dans un ouvrage de compte-rendu (proceedings), ou dans l'édition spéciale d'un journal reconnu (conference proceedings).
Sous-type
Poster: résume de manière illustrée et sur une page unique les résultats d'un projet de recherche. Les résumés de poster doivent être entrés sous "Abstract" et non "Poster".
Collection
Publications
Institution
UNIL/CHUV
Titre
Characterization of a major V3 duplication in the NS5A region of genotype 1b HCV by quasispecies analysis in a French multicenter study
Titre de la conférence
46th Annual Meeting of the European Association for the Study of the Liver (EASL)
Auteur⸱e⸱s
Le Guillou-Guillemette H., Bouthry E., Pivert A., Rosenberg A., Alain S., Thibault V., Abravanel F., Minjolle-Cha S., Andre-Garnier E., Moradpour D., Henquell C., Bour J.B., Petsaris O., Baazia Y., Andre P., Trimoulet P., Gaudy-Graffi C., Bettinger D., Saoudin H., Schvoerer E., Izopet J., Payan C., Lunel-Fabiani F.
Adresse
Berlin, Germany, March 30-April 3, 2011
ISBN
0168-8278
Statut éditorial
Publié
Date de publication
2011
Peer-reviewed
Oui
Volume
54
Série
Journal of Hepatology
Pages
S322
Langue
anglais
Notes
Publication type : Meeting Abstract
Résumé
Background and Aims: The NS5A protein of the HCV is known tobe involved in viral replication and assembly and probably in theresistance to Interferon based-therapy. Previous studies identifiedinsertions or deletions from 1 to 12 nucleotides in several genomicregions. In a multicenter study (17 French and 1 Swiss laboratoriesof virology), we identified for the first time a 31 amino acidsinsertion leading to a duplication of the V3 domain in the NS5Aregion with a high prevalence. Quasispecies of each strain withduplication were characterized and the inserted V3 domain wasidentified.Methods: Between 2006 and 2008, 1067 patients chronicallyinfected with a 1b HCV were consecutively included in the study.We first amplified the V3 region by RT-PCR to detect duplication(919 samples successfully amplified). The entire NS5A region wasthen amplified, cloned and sequenced in strains bearing theduplication. V3 sequences (called R1 and R2) from each clonewere analyzed with BioEdit and compared to a V3 consensussequence (C) built from the Database Los Alamos Hepatitis C.Entropy was determined at each position.Results: V3 duplications were identified in 25 patients representinga prevalence of 2.72%. We sequenced 2043 clones from which776 had a complete coding NS5A sequence (corresponding toa mean of 30 clones per patient). At the intra-individual level,6 to 17 variants were identified per V3 region, with a maximum of3 different amino acids. At the inter-individual level, a differenceof 7 and 2 amino acids was observed between C and R1 and R2sequences, respectively. Moreover few positions presented entropyhigher than 1 (4 for the R1, 2 for the R2 and 2 for the C). Among allthe sequenced clones, more than 60% were defective virus (partialfragment of NS5A or stop codon).Conclusions: We identified a duplication of the V3 domain ingenotype 1b HCV with a high prevalence. The R2 domain, which wasthe most similar to the C region, might probably be the "original"domain, whereas R1 should be the inserted domain. Phylogeneticanalyses are under process to confirm this hypothesis.
Mots-clé
,
OAI-PMH
oai:serval.unil.ch:BIB_7F3A5A70D8E4
Web of science
000297625601380
Création de la notice
03/01/2012 14:36
Dernière modification de la notice
20/08/2019 15:40
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