Your search keyword '"Eterradossi, Nicolas"' showing total 11 results

1. High antigenic diversity of serotype 1 infectious bursal disease virus revealed by antigenic cartography

Author

Cubas-Gaona, Liliana L., Courtillon, Céline, Briand, Francois-Xavier, Cotta, Higor, Bougeard, Stephanie, Hirchaud, Edouard, Leroux, Aurélie, Blanchard, Yannick, Keita, Alassane, Amelot, Michel, Eterradossi, Nicolas, Tatár-Kis, Tímea, Kiss, Istvan, Cazaban, Christophe, Grasland, Béatrice, and Soubies, Sébastien Mathieu

Published

2023

2. An alternative method to determine the 5′ extremities of non-segmented, negative sense RNA viral genomes using positive replication intermediate 3′ tailing: Application to two members of the Paramyxoviridae family

Author

Brown, Paul A., Briand, Francois-Xavier, Guionie, Olivier, Lemaitre, Evelyne, Courtillon, Celine, Henry, Aurelie, Jestin, Véronique, and Eterradossi, Nicolas

Published

2013

3. Infectious bursal disease virus in Algeria: Detection of highly pathogenic reassortant viruses.

Author

Abed, Mouna, Soubies, Sébastien, Courtillon, Céline, Briand, François-Xavier, Allée, Chantal, Amelot, Michel, De Boisseson, Claire, Lucas, Pierrick, Blanchard, Yannick, Belahouel, Ali, Kara, Redouane, Essalhi, Abdelhalim, Temim, Soraya, Khelef, Djamel, and Eterradossi, Nicolas

Subjects

*PATHOGENIC viruses, *IMMUNOSUPPRESSIVE agents, *VIRAL genomes, *MICROBIAL virulence, *MORTALITY

Abstract

Infectious bursal disease (IBD) is an immunosuppressive viral disease, present worldwide, which causes mortality and immunosuppression in young chickens. The causative agent, the Avibirnavirus IBDV, is a non-enveloped virus whose genome consists of two segments (A and B) of double-stranded RNA. Different pathotypes of IBDV exist, ranging from attenuated vaccine strains to very virulent viruses (vvIBDV). In Algeria, despite the prophylactic measures implemented, cases of IBD are still often diagnosed clinically and the current molecular epidemiology of IBDV remains unknown. The presence of the virus and especially of strains genetically close to vvIBDV was confirmed in 2000 by an unpublished OIE report. In this study, nineteen IBDV isolates were collected in Algeria between September 2014 and September 2015 during clinical outbreaks. These isolates were analyzed at the genetic, antigenic and pathogenic levels. Our results reveal a broad genetic and phenotypic diversity of pathogenic IBDV strains in Algeria, with, i) the circulation of viruses with both genome segments related to European vvIBDV, which proved as pathogenic for specific pathogen-free chickens as vvIBDV reference strain, ii) the circulation of viruses closely related - yet with a specific segment B - to European vvIBDV, their pathogenicity being lower than reference vvIBDV, iii) the detection of reassortant viruses whose segment A was related to vvIBDV whereas their segment B did not appear closely related to any reference sequence. Interestingly, the pathogenicity of these potentially reassortant strains was comparable to that of reference vvIBDV. All strains characterized in this study exhibited an antigenicity similar to the cognate reference IBDV strains. These data reveal the continuous genetic evolution of IBDV strains in Algerian poultry through reassortment and acquisition of genetic material of unidentified origin. Continuous surveillance of the situation as well as good vaccination practice associated with appropriate biosecurity measures are necessary for disease control. [ABSTRACT FROM AUTHOR]

Published

2018

4. Concomitant NA and NS deletion on avian Influenza H3N1 virus associated with hen mortality in France in 2019.

Author

Briand, François-Xavier, Schmitz, Audrey, Scoizec, Axelle, Allée, Chantal, Busson, Rachel, Guillemoto, Carole, Quenault, Hélène, Lucas, Pierrick, Pierre, Isabelle, Louboutin, Katell, Guillou-Cloarec, Cécile, Martenot, Claire, Cherbonnel-Pansart, Martine, Thomas, Rodolphe, Massin, Pascale, Souchaud, Florent, Blanchard, Yannick, Steensels, Mieke, Lambrecht, Benedicte, and Eterradossi, Nicolas

Subjects

*AVIAN influenza A virus, *AVIAN influenza, *COVID-19, *AGRICULTURAL exhibitions, *POULTRY farms, *HENS, *MORTALITY

Abstract

An H3N1 avian influenza virus was detected in a laying hens farm in May 2019 which had experienced 25% mortality in Northern France. The complete sequencing of this virus showed that all segment sequences belonged to the Eurasian lineage and were phylogenetically very close to many of the Belgian H3N1 viruses detected in 2019. The French virus presented two genetic particularities with NA and NS deletions that could be related to virus adaptation from wild to domestic birds and could increase virulence, respectively. Molecular data of H3N1 viruses suggest that these two deletions occurred at two different times. • Avian Influenza H3N1 virus detected in poultry farm exhibited mortality in France. • Concomitant NA and NS deletion on French avian Influenza H3N1 virus. • tMRCA analyses suggest two independent event dates for the occurrence of NA and NS deletions. [ABSTRACT FROM AUTHOR]

Published

2022

5. Genetic, antigenic and pathogenic characterization of four infectious bursal disease virus isolates from China suggests continued evolution of very virulent viruses.

Author

Li, Kai, Courtillon, Céline, Guionie, Olivier, Allée, Chantal, Amelot, Michel, Qi, Xiaole, Gao, Yulong, Wang, Xiaomei, and Eterradossi, Nicolas

Subjects

*VIRAL disease prevention, *VIRAL evolution, *NUCLEOTIDE sequence, *MONOCLONAL antibodies

Abstract

Infectious bursal disease virus (IBDV) causes an economically significant disease of young chickens worldwide. The emergence of very virulent IBDV (vvIBDV) strains has brought more challenges for effective prevention and control of this disease. The aim of the present study was to characterize four IBDV isolates from various regions of China between late 1990s and recent years and to compare them with previously isolated European IBDV strains. In this study, one Chinese vvIBDV strain isolated in 1999 and three strains isolated between 2005 and 2011 were analyzed at the genetic, antigenic and pathogenic levels. Strain SH99 was closely related and clustered in the same genetic lineage as the typical vvIBDV based on the genomic sequences of segments A and B. However, the three more recent Chinese vvIBDV (HLJ0504, HeB10 and HuN11) showed several genetic changes in both segments and clustered in a distinct lineage from the typical vvIBDV and the previously known Chinese vvIBDV. Based on the binding to a panel of neutralizing monoclonal antibodies in antigen capture enzyme-linked immunosorbent assays, all Chinese vvIBDVs exhibited similar antigenicity with the European typical vvIBDV strains. Nonetheless, the pathogenicity caused by the recent Chinese vvIBDV was higher than that induced by the European typical vvIBDV. This study calls for a sustained surveillance of IBD situation in China in order to support a better prevention and control of the disease. [ABSTRACT FROM AUTHOR]

Published

2015

6. Effect of in-feed paromomycin supplementation on antimicrobial resistance of enteric bacteria in turkeys.

Author

Kempf, Isabelle, Le Roux, Aurélie, Perrin-Guyomard, Agnès, Mourand, Gwenaëlle, Le Devendec, Laetitia, Bougeard, Stéphanie, Richez, Pascal, Le Pottier, Gilles, and Eterradossi, Nicolas

Subjects

*ANTI-infective agents, *DRUG resistance in bacteria, *NEOMYCIN, *TURKEYS, *AMINOGLYCOSIDES, *GUT microbiome, *DISEASES

Abstract

Histomoniasis in turkeys can be prevented by administering paromomycin sulfate, an aminoglycoside antimicrobial agent, in feed. The aim of this study was to evaluate the impact of in-feed paromomycin sulfate supplementation on the antimicrobial resistance of intestinal bacteria in turkeys. Twelve flocks of breeder turkeys were administered 100 ppm paromomycin sulfate from hatching to day 120; 12 flocks not supplemented with paromomycin were used as controls. Faecal samples were collected monthly from days 0 to 180. The resistance of Escherichia coli, Enterococcus faecium and Staphylococcus aureus to paramomycin and other antimicrobial agents was compared in paromomycin supplemented (PS) and unsupplemented (PNS) flocks. E.coli from PS birds had a significantly higher frequency of resistance to paromomycin, neomycin and kanamycin until 1 month after the end of supplementation compared to PNS birds. Resistance to amox-icillin or trimethoprim-sulfamethoxazole was also more frequent in PS turkeys. Resistance was mainly due to the presence of aph genes, which could be transmitted by conjugation, sometimes with strepto-mycin, tetracycline, amoxicillin, trimethoprim or sulfonamide resistance genes. Resistance to kanamycin and streptomycin in E. faecium was significantly different in PS and PNS breeders on days 60 and 90. Sig-nificantly higher frequencies of resistance to paromomycin, kanamycin, neomycin and tobramycin were observed in S. aureus isolates from PS birds. Paromomycin supplementation resulted in resistance to ami-noglycosides in bacteria of PS turkeys. Co-selection for resistance to other antimicrobial agents was observed in E. coli isolates [ABSTRACT FROM AUTHOR]

Published

2013

7. Generation of serotype 1/serotype 2 reassortant viruses of the infectious bursal disease virus and their investigation in vitro and in vivo

Author

Zierenberg, Kati, Raue, Rüdiger, Nieper, Hermann, Islam, Md. Rafiqul, Eterradossi, Nicolas, Toquin, Didier, and Müller, Hermann

Subjects

*GENETICS, *VIRAL replication, *ANIMAL orientation, *GENOMES

Abstract

Infectious bursal disease virus (IBDV) is the causative agent of acute or immunosuppressive disease in chickens. Serotype 1 strains are pathogenic whereas serotype 2 strains neither cause disease nor protect against infection with the serotype 1 strains. The target organ of serotype 1 strains is the bursa Fabricii (BF). The molecular determinants of this tropism, and therefore pathogenicity, are poorly understood. IBDV is a non-enveloped icosahedral virus particle of 60 nm in diameter, which contains two genome segments of double-stranded RNA. Here, the generation of interserotypic reassortants using the reverse genetics approach is reported. The results of in vitro and in vivo investigations show that genome segment A determines the bursa tropism of IBDV, whereas segment B is involved in the efficiency of viral replication; they further indicate the significance of the interaction of the polymerase (segment B) with the structural protein VP3 (segment A) or the viral genome for efficient virus formation and replication. [Copyright &y& Elsevier]

Published

2004

8. Avian adenovirus CELO recombinants expressing VP2 of infectious bursal disease virus induce protection against bursal disease in chickens

Author

Francois, Achille, Chevalier, Christophe, Delmas, Bernard, Eterradossi, Nicolas, Toquin, Didier, Rivallan, Gaëlle, and Langlois, Patrick

Subjects

*VIRUSES, *CHICKENS, *DNA, *VACCINATION

Abstract

To develop a CELO virus vector that can induce protection against infectious bursal disease, CELO viruses expressing the host-protective antigen VP2 of infectious bursal disease virus (IBDV) were constructed. In the engineered recombinants, the VP2 gene (the 441-first codons of the IBDA polyprotein) was placed under the control of the CMV promoter. Two positions in the CELO genome were chosen to insert the VP2 expression cassette. The recombinants were found apathogenic, when inoculated by different routes and even at high doses (up to 108 per animal). Chickens vaccinated oro-nasally with these different recombinants and challenged with very virulent IBDV were found to be poorly protected. In contrast, when inoculated with one or two (subcutaneous or intradermic) injections of CELOa-VP2, the chickens showed no clinical signs and no mortality after challenge. In the vaccinated chickens, the titers of neutralization antibody reached 7–9 values, showing that protection could be explained by the induction of a sufficient humoral response. After challenge, the weight ratio Bursa of Fabricius/body was about 2.5‰, a value similar to that obtained with the commercial Bur706 vaccine. However, histological lesions in the Bursa of Fabricius were observed, showing that a complete protection was not totally achieved. Contact transmission was evidenced. Protection was also obtained when inoculation of CELOa-VP2 was carried out in ovo. Prime-boost strategies were also tested with the CELOa-VP2 vector used in association with the purified VP2 antigen, or DNA encoding VP2 or a CELO vector expressing chicken myeloid growth factor (cMGF). None of these regimens were shown to substantially increase the level of protection when compared to double CELOa-VP2 inoculations. These results indicate that CELO-based vectors are useful to safely induce a strong protective immunity against vvIBDV in chickens. [Copyright &y& Elsevier]

Published

2004

9. Viral variant visualizer (VVV): A novel bioinformatic tool for rapid and simple visualization of viral genetic diversity.

Author

Flageul, Alexandre, Lucas, Pierrick, Hirchaud, Edouard, Touzain, Fabrice, Blanchard, Yannick, Eterradossi, Nicolas, Brown, Paul, and Grasland, Béatrice

Subjects

*PORCINE epidemic diarrhea virus, *RAPID tooling, *AVIAN infectious bronchitis virus, *MOLECULAR cloning, *VIRAL genomes

Abstract

• Processing NGS data to determine the composition of the viral population. • Visual description of a viral population as a variant map. • Easy to use bioinformatic pipeline on Galaxy instance. Here a bioinformatic pipeline VVV has been developed to analyse viral populations in a given sample from Next Generation Sequencing (NGS) data. To date, handling large amounts of data from NGS requires the expertise of bioinformaticians, both for data processing and result analysis. Consequently, VVV was designed to help non-bioinformaticians to perform these tasks. By providing only the NGS data file, the developed pipeline generated consensus sequences and determined the composition of the viral population for an avian Metapneumovirus (AMPV) and three different animal coronaviruses (Porcine Epidemic Diarrhea Virus (PEDV), Turkey Coronavirus (TCoV) and Infectious Bronchitis Virus (IBV)). In all cases, the pipeline produced viral consensus genomes corresponding to known consensus sequence and made it possible to highlight the presence of viral genetic variants through a single graphic representation. The method was validated by comparing the viral populations of an AMPV field sample, and of a copy of this virus produced from a DNA clone. VVV demonstrated that the cloned virus population was homogeneous (as designed) at position 2934 where the wild-type virus demonstrated two variant populations at a ratio of almost 50:50. A total of 18, 10, 3 and 28, viral genetic variants were detected for AMPV, PEDV, TCoV and IBV respectively. The simplicity of this pipeline makes the study of viral genetic variants more accessible to a wide variety of biologists, which should ultimately increase the rate of understanding of the mechanisms of viral genetic evolution. [ABSTRACT FROM AUTHOR]

Published

2021

10. Genetic diversity and evolution of Hare Calicivirus (HaCV), a recently identified lagovirus from Lepus europaeus.

Author

Droillard, Clément, Lemaitre, Evelyne, Chatel, Marina, Quéméner, Agnès, Briand, François-Xavier, Guitton, Jean-Sébastien, Marchandeau, Stéphane, Le Pendu, Jacques, Eterradossi, Nicolas, and Le Gall-Reculé, Ghislaine

Subjects

*CALICIVIRUSES, *HARES, *CYTOSKELETAL proteins, *PATHOGENIC viruses, *PROTEIN models

Abstract

First recognized as highly pathogenic viruses, hare lagoviruses belonging to genotype GII.1 (EBHSV) infect various Lepus species. Genetically distinct benign lagoviruses (Hare Calicivirus, HaCV) have recently been identified but few data have been available so far on these strains. The analysis of 199 samples from hunted hares collected throughout France allowed the detection of 20 HaCV and showed that they were widely distributed in this country. Ten HaCV capsid protein gene sequences were characterized. A first HaCV capsid protein structural model was proposed, revealing a global structure similar to that of a pathogenic GII.1 strain. The HaCV sequences showed an even higher genetic diversity than previously appreciated, with the characterization of two genotypes (GII.2, GII.3) and several additional putative genotypes. The most recent common ancestor for HaCV VP60 gene was estimated to be much older than that for GII.1 pathogenic strains. These results give new insights into the phylogenetic relationships of HaCV within the Lagovirus genus. • Ten new HaCV capsid protein VP60 gene sequences described • Characterization of two new genotypes and several putative genotypes • First capsid protein structural model proposed for a benign lagovirus • TMRCA for HaCV capsid protein gene estimated long before that of pathogenic strains • Probable common genetic origin of European and Australian HaCV [ABSTRACT FROM AUTHOR]

Published

2020

11. Continuous circulation of an antigenically modified very virulent infectious bursal disease virus for fifteen years in Egypt.

Author

Samy, Ahmed, Courtillon, Céline, Briand, François-Xavier, Khalifa, Mohamed, Selim, Abdullah, Arafa, Abd El Satar, Hegazy, Ahmed, Eterradossi, Nicolas, and Soubies, Sébastien M.

Subjects

*INFECTIOUS bursal disease virus, *CHICKEN diseases, *BROILER chickens, *TISSUE culture

Abstract

Infectious bursal disease virus (IBDV), the agent of an immunosuppressive and sometimes lethal disease in chickens, is causing recurrent outbreaks in broiler chickens in Egypt. In particular, an antigenically modified isolate of very virulent IBDV (vvIBDV) called 99323 was detected in Egypt nearly twenty years ago; this isolate was shown to be experimentally controlled by an antigenically classical live vaccine. However, acute IBD is still reported, even in vaccinated flocks, and little is known about the genetic and antigenic properties of viruses currently circulating in Egypt. In the present study, ten samples collected in Egyptian broiler farms in 2015 as well as five samples collected in 2001 were analyzed. Genetic analyses of partial VP2 sequences revealed that 8 isolates clustered with vvIBDV strains, and 5 with tissue culture adapted and vaccine strains. Similar results were observed for partial VP1 sequences with the exception of isolate 160019, for which VP2 clustered with the vaccine strain Bursine while VP1 clustered with vvIBDV, suggesting reassortment. For isolates genetically related to vvIBDV, antigenic profiling revealed two patterns: while some isolates exhibited typical European vvIBDV reactivity with lack of binding of mAbs 5, other revealed extensive antigenic modifications, with lack of binding of mAbs 3, 5, 6, 8 and 9, similar to isolate 99323. These different patterns were associated with a single amino acid mutation at position 321 of VP2 that is located within peak P HI. Full genome sequencing was performed for three isolates, among which two were representative of the two antigenic patterns observed for vvIBDV as well as the reassortant isolate 160019. This study highlights the co-circulation of both antigenically typical and modified vvIBDV during the last fifteen years in Egypt. • Antigenically atypical very virulent IBDV (vvIBDV) are detected in Egypt. • These viruses have persisted for 15 years in Egypt. • Antigenically atypical and typical vvIBDV co-circulate in Egypt. [ABSTRACT FROM AUTHOR]

Published

2020