Your search keyword '"Briones C"' showing total 7 results

1. High-Resolution Hepatitis C Virus Subtyping Using NS5B Deep Sequencing and Phylogeny, an Alternative to Current Methods

Author

Xavier Forns, Marta Bes, Javier García-Samaniego, Manuel Romero-Gómez, Rafael Esteban, Josep Gregori, Maria Buti, Julie Sheldon, Silvia Sauleda, Sofía Pérez-del-Pulgar, Maria Homs, Miguel Álvarez-Tejado, Celia Perales, David Tabernero, Rosa Quiles-Pérez, L Viladomiu, Jose Antonio delCampo, Jordi Gómez, Carlos Briones, Antonio Madejón, Sabela Lens, Jose Manuel Muñoz, Maria Blasi, Francisco Rodriguez-Frias, Lluis Castells, Rosario López-Rodríguez, Maria Cubero, Jaume Guardia, Rosario Casillas, Josep Quer, Andrea Caballero, Damir Garcia-Cehic, Paloma Muñoz-de-Rueda, Paloma Sanz-Cameno, Juan Ignacio Esteban, Javier Salmerón, Irene Belmonte, Helena Allende, Ricardo Moreno-Otero, L. Nieto, Angela Ruiz-Extremera, Esteban Domingo, [Quer,J, Gregori,J, Buti,M, Garcia-Cehic,D, Cubero,M, Castells,L, Viladomiu,L, Guardia,J, Esteban,R, Esteban,JI] Liver Unit, Internal Medicine, Lab. Malalties Hepàtiques, Vall d'Hebron Institut Recerca—Hospital Universitari Vall d'Hebron (VHIR-HUVH), Barcelona, Spain. [Quer,J, Rodríguez-Friaas,F, Madejon,A, Perez-del-Pulgar,S, Casillas,R, Blasi,M, Homs,M, Tabernero,D, Cubero, del Campo,JA, Domingo,E, Lens,S, Muñoz-de-Rueda,P, Sanz-Cameno,P, Sauleda,S, Bes,M, Gomez,J, Briones,C, Perales,C, Sheldon,J, Salmeron,J, Ruiz-Extremera,A, Quiles-Pérez,R, Moreno-Otero,R, López-Rodríguez,R, Romero-Gómez,M, Garcia-Samaniego,J, Forns,X, Esteban,JI] Centro de Investigación Biomédica en Red (CIBER) de Enfermedades Hepáticas y Digestivas (CIBERehd) del Instituto de Salud Carlos III, Madrid, Spain. [Quer,J, Rodríguez-Frias,F, Esteban,JI] Universitat Autònoma de Barcelona, Barcelona, Spain. [Gregori,J, Alvarez-Tejado,M, Muñoz,JM] Roche Diagnostics SL, Barcelona, Spain. [Rodrígue-Frias,F, Casilla,R, Caballero,A, Belmonte,I, Nieto,L] Biochemistry Unit, Virology Unit /Microbiology Department, HUVH, Barcelona, Spain. [Madejo,A, Garcia-Samaniego,J] Liver Unit, Hospital La Paz-Carlos III, Madrid, Spain. [Perez-del-Pulgar,S, Forns,X] Liver Unit, Hospital Clinic, IDIBAPS, Barcelona, Spain. [del Campo,JA, Romero-Gomez,M] Hospital Universitario Virgen de Valme, Seville, Spain.[Domingo,E, Sheldon,J] Centro de Biología Molecular Severo Ochoa-Universidad Autónoma de Madrid (CSIC-UAM), Campus de Cantoblanco, Madrid, Spain. [Muñoz-de-Rueda,P, Ruiz Extremera,A, Quiles-Pérez,R] Hospital San Cecilio, Granada, Spain. [San-Cameno,P, López-Rodríguez,R] Hospital de la Princesa, Madrid, Spain. [Sauleda,S, Bes,M] Banc de Sang i de Teixits, Institut Català de la Salut, Barcelona, Spain. [Gomez,J] CSIC, Instituto de Parasitología y Biomedicina López Neyra, Granada, Spain. [Briones,C] Centro de Astrobiología (CSIC-INTA), Madrid, Spain. [Allende,H] Pathological Anatomy Department, VHIR-HUVH, Barcelona, Spain., This study has been supported by CDTI (Centro para el Desarrollo Tecnológico Industrial), Spanish Ministry of Economics and Competitiveness (MINECO), IDI-20110115, MINECO projects SAF 2009-10403, and also by the Spanish Ministry of Health, Instituto de Salud Carlos III (FIS) projects PI10/01505, PI12/01893, and PI13/00456. CIBERehd is funded by the Instituto de Salud Carlos III, Madrid, Spain. Work at CBMSO was supported by grant MINECO-BFU2011-23604, FIPSE and Fundación Ramón Areces., UAM. Departamento de Medicina, Centro de Biología Molecular Severo Ochoa (CBM), Centro para el Desarrollo Tecnológico Industrial (España), Ministerio de Economía y Competitividad (España), Ministerio de Sanidad y Consumo (España), Fundación para la Investigación y la Prevención del Sida en España, Fundación Ramón Areces, and Instituto de Salud Carlos III

Subjects

Microbiology (medical), Genotyping Techniques, Genotype, Medicina, Hepatitis C virus, Population, Organisms::Viruses::Hepatitis Viruses::Hepacivirus [Medical Subject Headings], Diseases::Virus Diseases::Hepatitis, Viral, Human::Hepatitis C [Medical Subject Headings], Chemicals and Drugs::Chemical Actions and Uses::Specialty Uses of Chemicals::Laboratory Chemicals::Indicators and Reagents::Reagent Kits, Diagnostic [Medical Subject Headings], Hepacivirus, Biology, Viral Nonstructural Proteins, medicine.disease_cause, Deep sequencing, Técnicas de genotipaje, Organisms::Eukaryota::Animals::Chordata::Vertebrates::Mammals::Primates::Haplorhini::Catarrhini::Hominidae::Humans [Medical Subject Headings], chemistry.chemical_compound, symbols.namesake, Proteínas no estructurales virales, Virology, medicine, Humans, Chemicals and Drugs::Amino Acids, Peptides, and Proteins::Proteins::Viral Proteins::Viral Nonstructural Proteins [Medical Subject Headings], education, NS5B, Genotyping, Phylogeny, Sanger sequencing, education.field_of_study, Analytical, Diagnostic and Therapeutic Techniques and Equipment::Investigative Techniques::Genetic Techniques::Genotyping Techniques [Medical Subject Headings], High-Throughput Nucleotide Sequencing, Antivirals, Hepatitis C, Subtyping, Author Corrections, Humanos, Juego de reactivos para diagnóstico, Filogenia, chemistry, HCV, symbols, Phenomena and Processes::Genetic Phenomena::Phylogeny [Medical Subject Headings], Phenomena and Processes::Genetic Phenomena::Genotype [Medical Subject Headings], Reagent Kits, Diagnostic

Abstract

All Rights Reserved. HepatitisCvirus(HCV)is classified into seven major genotypesand67 subtypes. Recent studies haveshownthat inHCVgenotype 1-infected patients, response rates to regimens containingdirect-acting antivirals(DAAs)are subtype dependent. Currently available genotypingmethods have limited subtyping accuracy.Wehave evaluated theperformanceof adeep-sequencing-basedHCVsubtyping assay, developed for the 454/GS-Junior platform, in comparisonwith thoseof two commercial assays (VersantHCVgenotype 2.0andAbbott Real-timeHCVGenotype II)andusingdirectNS5Bsequencing as a gold standard (direct sequencing), in 114 clinical specimenspreviously tested by first-generation hybridization assay (82 genotype 1and32 with uninterpretable results). Phylogenetic analysis of deep-sequencing reads matched subtype 1 callingbypopulation Sanger sequencing(69%1b,31%1a) in 81 specimensandidentified amixed-subtype infection (1b/3a/1a) in one sample. Similarly,amongthe 32previously indeterminate specimens, identical genotypeandsubtype results were obtained by directanddeep sequencing in all but four samples with dual infection. In contrast, both VersantHCVGenotype 2.0andAbbott Real-timeHCVGenotype II failed subtype 1 calling in 13 (16%) samples eachandwere unable to identify theHCVgenotype and/or subtype inmore than half of the nongenotype 1 samples.Weconcluded that deep sequencing ismore efficient forHCVsubtyping than currently available methodsandallows qualitative identificationofmixed infectionsandmay bemorehelpfulwith respect to informing treatment strategies withnewDAA-containing regimens across allHCVsubtypes., This study has been supported by CDTI (Centro para el Desarrollo Tecnológico Industrial), Spanish Ministry of Economics and Competitiveness (MINECO), IDI-20110115; MINECO projects SAF 2009-10403; and also by the Spanish Ministry of Health, Instituto de Salud Carlos III (FIS) projects PI10/01505, PI12/01893, and PI13/00456. CIBERehd is funded by the Instituto de Salud Carlos III, Madrid, Spain. Work at CBMSO was supported by grant MINECO-BFU2011-23604, FIPSE, and Fundación Ramón Areces.

Published

2014

2. Broad and dynamic diversification of infectious hepatitis c virus in a cell culture environment

Author

Josep Quer, Qian Chen, Ana Isabel de Ávila, Irene Sanchez-Martin, Celia Perales, Isabel Gallego, Inés Palacios-Blanco, Jordi Gómez, María Eugenia Soria, Brenda Martínez-González, Damir Garcia-Cehic, Soumaya Khalfaoui, Josep Gregori, Patricia Martínez-Barragán, Carlos Briones, Esteban Domingo, Juan Ignacio Esteban, Carlos García-Crespo, Eugenia Soria, M. [0000-0003-1755-6382], García Crespo, C. [0000-0001-6561-5389], García Cehic, D. [0000-0002-0009-038X], Briones, C. [0000-0003-2213-8353], Domingo, E. [0000-0002-0573-1676], Martínez González, B. [0000-0002-4482-5181], Perales Viejo, C. B. [0000-0003-1618-1937], Gregori Font, J. [0000-0002-4253-8015], Gómez, J. [0000-0002-7806-1503], Quer, J. [0000-0003-0014-084X], Instituto de Salud Carlos III (ISCIII), Comunidad de Madrid, Ministerio de Economia y Competitividad (MINECO), Fundación Ramón Areces, Banco Santander, Agencia Estatal de Investigación (AEI), Ministerio de Ciencia Innovación y Universidades (MICIU), Miguel Servet program of the Instituto de Salud Carlos III, European Regional Development Fund (ERDF), Centro para el Desarrollo Tecnologico Industrial (CDTI) from the Spanish Ministry of Economy and Business, Unidad de Excelencia Científica María de Maeztu Centro de Astrobiología del Instituto Nacional de Técnica Aeroespacial y CSIC, Comunidad de Madrid [CAM]/FEDER, Ministerio de Economía y Competitividad (España), Ministerio de Ciencia, Innovación y Universidades (España), Instituto de Salud Carlos III, European Commission, Agencia Estatal de Investigación (España), and Ministerio de Economía y Empresa (España)

Subjects

Mutation rate, Immunology, Mutant, Population, Cell Culture Techniques, Viral quasispecies, Hepacivirus, adaptation, Virus Replication, Microbiology, Genome, Virus, 03 medical and health sciences, Virology, Cell Line, Tumor, Humans, education, 030304 developmental biology, Genetics, 0303 health sciences, education.field_of_study, biology, 030306 microbiology, mutational waves, RNA virus, mutant spectrum, biology.organism_classification, Phenotype, Adaptation, Physiological, Genetic Diversity and Evolution, sequence space, Insect Science, Mutation, RNA virus evolution

Abstract

Previous studies documented that long-term hepatitis C virus (HCV) replication in human hepatoma Huh-7.5 cells resulted in viral fitness gain, expansion of the mutant spectrum, and several phenotypic alterations. In the present work, we show that mutational waves (changes in frequency of individual mutations) occurred continuously and became more prominent as the virus gained fitness. They were accompanied by an increasing proportion of heterogeneous genomic sites that affected 1 position in the initial HCV population and 19 and 69 positions at passages 100 and 200, respectively. Analysis of biological clones of HCV showed that these dynamic events affected infectious genomes, since part of the fluctuating mutations became incorporated into viable genomes. While 17 mutations were scored in 3 biological clones isolated from the initial population, the number reached 72 in 3 biological clones from the population at passage 200. Biological clones differed in their responses to antiviral inhibitors, indicating a phenotypic impact of viral dynamics. Thus, HCV adaptation to a specific constant environment (cell culture without external influences) broadens the mutant repertoire and does not focus the population toward a limited number of dominant genomes. A retrospective examination of mutant spectra of foot-and-mouth disease virus passaged in cell cultures suggests a parallel behavior here described for HCV. We propose that virus diversification in a constant environment has its basis in the availability of multiple alternative mutational pathways for fitness gain. This mechanism of broad diversification should also apply to other replicative systems characterized by high mutation rates and large population sizes. IMPORTANCE The study shows that extensive replication of an RNA virus in a constant biological environment does not limit exploration of sequence space and adaptive options. There was no convergence toward a restricted set of adapted genomes. Mutational waves and mutant spectrum broadening affected infectious genomes. Therefore, profound modifications of mutant spectrum composition and consensus sequence diversification are not exclusively dependent on environmental alterations or the intervention of population bottlenecks., The work at CBMSO was supported by grants SAF2014-52400-R from Ministerio de Economía y Competitividad (MINECO); SAF2017-87846-R and BFU2017-91384-EXP from Ministerio de Ciencia, Innovación y Universidades (MICIU); and S2013/ABI-2906 (PLATESA from Comunidad de Madrid [CAM]/FEDER), S2018/BAA-4370 (PLATESA2 from CAM/FEDER), and PI18/00210 from Instituto de Salud Carlos III. C.P. is supported by the Miguel Servet program of the Instituto de Salud Carlos III (CP14/00121), cofinanced by the European Regional Development Fund (ERDF). CIBERehd is funded by Instituto de Salud Carlos III. Institutional grants from the Fundación Ramón Areces and Banco Santander to the CBMSO are also acknowledged. The team at CBMSO belongs to the Global Virus Network (GVN). The work in Barcelona was supported by Instituto de Salud Carlos III, cofinanced by the European Regional Development Fund (ERDF) (grant numbers PI16/00337) and by the Centro para el Desarrollo Tecnológico Industrial (CDTI) from the Spanish Ministry of Economy and Business (grant number IDI-20151125). Work at CAB was supported by MINECO grant BIO2016-79618-R (funded by the European Union under the FEDER program) and by the Spanish State Research Agency (AEI) through project number MDM-2017-0737 Unidad de Excelencia “María de Maeztu”-Centro de Astrobiologia (CSIC-INTA).

Published

2020

3. Fitness-Dependent, Mild Mutagenic Activity of Sofosbuvir for Hepatitis C Virus.

Author

Martínez-González B, Gallego I, Gregori J, Soria ME, Somovilla P, de Ávila AI, García-Crespo C, Durán-Pastor A, Briones C, Gómez J, Quer J, Domingo E, and Perales C

Subjects

Humans, Sofosbuvir pharmacology, Sofosbuvir therapeutic use, Hepacivirus genetics, Mutagens pharmacology, Antiviral Agents pharmacology, Antiviral Agents therapeutic use, Genotype, Ribavirin therapeutic use, Treatment Outcome, Drug Therapy, Combination, Hepatitis C drug therapy, Hepatitis C, Chronic drug therapy

Abstract

The concept of a mild mutagen was coined to describe a minor mutagenic activity exhibited by some nucleoside analogues that potentiated their efficacy as antiretroviral agents. In the present study, we report the mild mutagen activity of sofosbuvir (SOF) for hepatitis C virus (HCV). Serial passages of HCV in human hepatoma cells, in the presence of SOF at a concentration well below its cytotoxic concentration 50 (CC 50 ) led to pre-extinction populations whose mutant spectra exhibited a significant increase of C→U transitions, relative to populations passaged in the absence of SOF. This was reflected in an increase in several diversity indices that were used to characterize viral quasispecies. The mild mutagenic activity of SOF was largely absent when it was tested with isogenic HCV populations that displayed high replicative fitness. Thus, SOF can act as a mild mutagen for HCV, depending on HCV fitness. Possible mechanisms by which the SOF mutagenic activity may contribute to its antiviral efficacy are discussed.

Published

2023

4. Amino Acid Substitutions Associated with Treatment Failure for Hepatitis C Virus Infection.

Author

Soria ME, García-Crespo C, Martínez-González B, Vázquez-Sirvent L, Lobo-Vega R, de Ávila AI, Gallego I, Chen Q, García-Cehic D, Llorens-Revull M, Briones C, Gómez J, Ferrer-Orta C, Verdaguer N, Gregori J, Rodríguez-Frías F, Buti M, Esteban JI, Domingo E, Quer J, and Perales C

Subjects

Amino Acid Substitution, Antiviral Agents pharmacology, Antiviral Agents therapeutic use, Drug Resistance, Viral genetics, Genotype, Hepacivirus genetics, Humans, Treatment Failure, Viral Nonstructural Proteins genetics, Hepatitis C drug therapy, Hepatitis C, Chronic drug therapy

Abstract

Despite the high virological response rates achieved with current directly acting antiviral agents (DAAs) against hepatitis C virus (HCV), around 2% to 5% of treated patients do not achieve a sustained viral response. The identification of amino acid substitutions associated with treatment failure requires analytical designs, such as subtype-specific ultradeep sequencing (UDS) methods, for HCV characterization and patient management. Using this procedure, we have identified six highly represented amino acid substitutions (HRSs) in NS5A and NS5B of HCV, which are not bona fide resistance-associated substitutions (RAS), from 220 patients who failed therapy. They were present frequently in basal and posttreatment virus of patients who failed different DAA-based therapies. Contrary to several RAS, HRSs belong to the acceptable subset of substitutions according to the PAM250 replacement matrix. Their mutant frequency, measured by the number of deep sequencing reads within the HCV quasispecies that encode the relevant substitutions, ranged between 90% and 100% in most cases. They also have limited predicted disruptive effects on the three-dimensional structures of the proteins harboring them. Possible mechanisms of HRS origin and dominance, as well as their potential predictive value for treatment response, are discussed., (Copyright © 2020 American Society for Microbiology.)

Published

2020

5. Broad and Dynamic Diversification of Infectious Hepatitis C Virus in a Cell Culture Environment.

Author

Gallego I, Soria ME, García-Crespo C, Chen Q, Martínez-Barragán P, Khalfaoui S, Martínez-González B, Sanchez-Martin I, Palacios-Blanco I, de Ávila AI, García-Cehic D, Esteban JI, Gómez J, Briones C, Gregori J, Quer J, Perales C, and Domingo E

Subjects

Cell Line, Tumor, Humans, Adaptation, Physiological, Cell Culture Techniques, Hepacivirus physiology, Mutation, Virus Replication

Abstract

Previous studies documented that long-term hepatitis C virus (HCV) replication in human hepatoma Huh-7.5 cells resulted in viral fitness gain, expansion of the mutant spectrum, and several phenotypic alterations. In the present work, we show that mutational waves (changes in frequency of individual mutations) occurred continuously and became more prominent as the virus gained fitness. They were accompanied by an increasing proportion of heterogeneous genomic sites that affected 1 position in the initial HCV population and 19 and 69 positions at passages 100 and 200, respectively. Analysis of biological clones of HCV showed that these dynamic events affected infectious genomes, since part of the fluctuating mutations became incorporated into viable genomes. While 17 mutations were scored in 3 biological clones isolated from the initial population, the number reached 72 in 3 biological clones from the population at passage 200. Biological clones differed in their responses to antiviral inhibitors, indicating a phenotypic impact of viral dynamics. Thus, HCV adaptation to a specific constant environment (cell culture without external influences) broadens the mutant repertoire and does not focus the population toward a limited number of dominant genomes. A retrospective examination of mutant spectra of foot-and-mouth disease virus passaged in cell cultures suggests a parallel behavior here described for HCV. We propose that virus diversification in a constant environment has its basis in the availability of multiple alternative mutational pathways for fitness gain. This mechanism of broad diversification should also apply to other replicative systems characterized by high mutation rates and large population sizes. IMPORTANCE The study shows that extensive replication of an RNA virus in a constant biological environment does not limit exploration of sequence space and adaptive options. There was no convergence toward a restricted set of adapted genomes. Mutational waves and mutant spectrum broadening affected infectious genomes. Therefore, profound modifications of mutant spectrum composition and consensus sequence diversification are not exclusively dependent on environmental alterations or the intervention of population bottlenecks., (Copyright © 2020 American Society for Microbiology.)

Published

2020

6. Correction for Quer at al., High-Resolution Hepatitis C Virus Subtyping Using NS5B Deep Sequencing and Phylogeny, an Alternative to Current Methods.

Author

Quer J, Gregori J, Rodríguez-Frias F, Buti M, Madejon A, Perez-Del-Pulgar S, Garcia-Cehic D, Casillas R, Blasi M, Homs M, Tabernero D, Alvarez-Tejado M, Muñoz JM, Cubero M, Caballero A, delCampo JA, Domingo E, Belmonte I, Nieto L, Lens S, Muñoz-de-Rueda P, Sanz-Cameno P, Sauleda S, Bes M, Gomez J, Briones C, Perales C, Sheldon J, Castells L, Viladomiu L, Salmeron J, Ruiz-Extremera A, Quiles-Pérez R, Moreno-Otero R, López-Rodríguez R, Allende H, Romero-Gómez M, Guardia J, Esteban R, Garcia-Samaniego J, Forns X, and Esteban JI

Published

2016

7. High-resolution hepatitis C virus subtyping using NS5B deep sequencing and phylogeny, an alternative to current methods.

Author

Quer J, Gregori J, Rodríguez-Frias F, Buti M, Madejon A, Perez-del-Pulgar S, Garcia-Cehic D, Casillas R, Blasi M, Homs M, Tabernero D, Alvarez-Tejado M, Muñoz JM, Cubero M, Caballero A, del Campo JA, Domingo E, Belmonte I, Nieto L, Lens S, Muñoz-de-Rueda P, Sanz-Cameno P, Sauleda S, Bes M, Gomez J, Briones C, Perales C, Sheldon J, Castells L, Viladomiu L, Salmeron J, Ruiz-Extremera A, Quiles-Pérez R, Moreno-Otero R, López-Rodríguez R, Allende H, Romero-Gómez M, Guardia J, Esteban R, Garcia-Samaniego J, Forns X, and Esteban JI

Subjects

Genotyping Techniques, Hepatitis C diagnosis, Humans, Reagent Kits, Diagnostic, Genotype, Hepacivirus classification, Hepacivirus genetics, Hepatitis C virology, High-Throughput Nucleotide Sequencing, Phylogeny, Viral Nonstructural Proteins genetics

Abstract

Hepatitis C virus (HCV) is classified into seven major genotypes and 67 subtypes. Recent studies have shown that in HCV genotype 1-infected patients, response rates to regimens containing direct-acting antivirals (DAAs) are subtype dependent. Currently available genotyping methods have limited subtyping accuracy. We have evaluated the performance of a deep-sequencing-based HCV subtyping assay, developed for the 454/GS-Junior platform, in comparison with those of two commercial assays (Versant HCV genotype 2.0 and Abbott Real-time HCV Genotype II) and using direct NS5B sequencing as a gold standard (direct sequencing), in 114 clinical specimens previously tested by first-generation hybridization assay (82 genotype 1 and 32 with uninterpretable results). Phylogenetic analysis of deep-sequencing reads matched subtype 1 calling by population Sanger sequencing (69% 1b, 31% 1a) in 81 specimens and identified a mixed-subtype infection (1b/3a/1a) in one sample. Similarly, among the 32 previously indeterminate specimens, identical genotype and subtype results were obtained by direct and deep sequencing in all but four samples with dual infection. In contrast, both Versant HCV Genotype 2.0 and Abbott Real-time HCV Genotype II failed subtype 1 calling in 13 (16%) samples each and were unable to identify the HCV genotype and/or subtype in more than half of the non-genotype 1 samples. We concluded that deep sequencing is more efficient for HCV subtyping than currently available methods and allows qualitative identification of mixed infections and may be more helpful with respect to informing treatment strategies with new DAA-containing regimens across all HCV subtypes., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published

2015