Your search keyword '"Ortego J"' showing total 14 results

1. Co-expression of VP2, NS1 and NS2-Nt proteins by an MVA viral vector induces complete protection against bluetongue virus.

Author

Jiménez-Cabello L, Utrilla-Trigo S, Calvo-Pinilla E, Lorenzo G, Illescas-Amo M, Benavides J, Moreno S, Marín-López A, Nogales A, and Ortego J

Subjects

Animals, Mice, Mice, Knockout, Antibodies, Viral immunology, Antibodies, Viral blood, Antibodies, Neutralizing immunology, Antibodies, Neutralizing blood, Female, Bluetongue virus immunology, Bluetongue virus genetics, Viral Nonstructural Proteins immunology, Viral Nonstructural Proteins genetics, Bluetongue prevention & control, Bluetongue immunology, Bluetongue virology, Viral Vaccines immunology, Viral Vaccines genetics, Vaccinia virus genetics, Vaccinia virus immunology, Receptor, Interferon alpha-beta genetics, Genetic Vectors, Capsid Proteins immunology, Capsid Proteins genetics

Abstract

Introduction: Bluetongue (BT), caused by bluetongue virus (BTV), is an important arthropod-borne livestock disease listed by the World Organization for Animal Health. Live-attenuated and inactivated vaccines have permitted to control BT but they do not simultaneously protect against the myriad of BTV serotypes. Recently, we identified the highly conserved BTV nonstructural protein NS1 and the N-terminal region of NS2 as antigens capable of conferring multiserotype protection against BTV., Methods: Here, we designed Modified Vaccinia Ankara (MVA) viral vectors that expressed BTV-4 proteins VP2 or VP7 along with NS1 and NS2-Nt as well as MVAs that expressed proteins VP2, VP7 or NS1 and NS2-Nt., Results: Immunization of IFNAR(-/-) mice with two doses of MVA-NS1-2A-NS2-Nt protected mice from BTV-4M infection by the induction of an antigen-specific T cell immune response. Despite rMVA expressing VP7 alone were not protective in the IFNAR(-/-) mouse model, inclusion of VP7 in the vaccine formulation amplified the cell-mediated response induced by NS1 and NS2-Nt. Expression of VP2 elicited protective non-cross-reactive neutralizing antibodies (nAbs) in immunized animals and improved the protection observed in the MVA-NS1-2A-NS2-Nt immunized mice when these three BTV antigens were co-expressed. Moreover, vaccines candidates co-expressing VP2 or VP7 along with NS1 and NS2-Nt provided multiserotype protection. We assessed protective efficacy of both vaccine candidates in sheep against virulent challenge with BTV-4M., Discussion: Immunization with MVA-VP7-NS1-2A-NS2-Nt partially dumped viral replication and clinical disease whereas administration of MVA-VP2-NS1-2A-NS2-Nt promoted a complete protection, preventing viraemia and the pathology produced by BTV infection., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2024 Jiménez-Cabello, Utrilla-Trigo, Calvo-Pinilla, Lorenzo, Illescas-Amo, Benavides, Moreno, Marín-López, Nogales and Ortego.)

Published

2024

2. The Combined Expression of the Nonstructural Protein NS1 and the N-Terminal Half of NS2 (NS2 1-180 ) by ChAdOx1 and MVA Confers Protection against Clinical Disease in Sheep upon Bluetongue Virus Challenge.

Author

Utrilla-Trigo S, Jiménez-Cabello L, Calvo-Pinilla E, Marín-López A, Lorenzo G, Sánchez-Cordón P, Moreno S, Benavides J, Gilbert S, Nogales A, and Ortego J

Subjects

Animals, Antibodies, Neutralizing immunology, Antibodies, Viral immunology, Bluetongue virus classification, Genetic Vectors immunology, Immunity, Cellular, Immunization, Immunogenicity, Vaccine, Serogroup, Sheep, Vaccines, DNA genetics, Vaccines, DNA immunology, Vaccinia virus immunology, Viral Nonstructural Proteins immunology, Viral Vaccines administration & dosage, Viral Vaccines genetics, Bluetongue prevention & control, Bluetongue virus immunology, Genetic Vectors genetics, Vaccinia virus genetics, Viral Nonstructural Proteins genetics, Viral Vaccines immunology

Abstract

Bluetongue, caused by bluetongue virus (BTV), is a widespread arthropod-borne disease of ruminants that entails a recurrent threat to the primary sector of developed and developing countries. In this work, we report modified vaccinia virus Ankara (MVA) and ChAdOx1-vectored vaccines designed to simultaneously express the immunogenic NS1 protein and/or NS2-Nt, the N-terminal half of protein NS2 (NS2 1-180 ). A single dose of MVA or ChAdOx1 expressing NS1-NS2-Nt improved the protection conferred by NS1 alone in IFNAR(-/-) mice. Moreover, mice immunized with ChAdOx1/MVA-NS1, ChAdOx1/MVA-NS2-Nt, or ChAdOx1/MVA-NS1-NS2-Nt developed strong cytotoxic CD8 + T-cell responses against NS1, NS2-Nt, or both proteins and were fully protected against a lethal infection with BTV serotypes 1, 4, and 8. Furthermore, although a single immunization with ChAdOx1-NS1-NS2-Nt partially protected sheep against BTV-4, the administration of a booster dose of MVA-NS1-NS2-Nt promoted a faster viral clearance, reduction of the period and level of viremia and also protected from the pathology produced by BTV infection. IMPORTANCE Current BTV vaccines are effective but they do not allow to distinguish between vaccinated and infected animals (DIVA strategy) and are serotype specific. In this work we have develop a DIVA multiserotype vaccination strategy based on adenoviral (ChAdOx1) and MVA vaccine vectors, the most widely used in current phase I and II clinical trials, and the conserved nonstructural BTV proteins NS1 and NS2. This immunization strategy solves the major drawbacks of the current marketed vaccines.

Published

2022

3. Recombinant Modified Vaccinia Virus Ankara Development to Express VP2, NS1, and VP7 Proteins of Bluetongue Virus.

Author

Marín-López A, Utrilla-Trigo S, Jiménez-Cabello L, and Ortego J

Subjects

Animals, Capsid Proteins genetics, Mammals, Sheep, Vaccinia virus genetics, Bluetongue prevention & control, Bluetongue virus genetics, Viral Vaccines

Abstract

Modified vaccinia virus Ankara (MVA) is employed widely as an experimental vaccine vector for its abortive replication in mammalian cells and high expression level of foreign/heterologous genes. Recombinant MVAs (rMVAs) are used as platforms for protein production as well as vectors to generate vaccines against a wide range of infectious diseases and other pathologies. The portrait of the virus combines desirable elements such as high-level biological safety, the ability to activate appropriate innate immune mediators upon vaccination , and the capacity to deliver substantial amounts of heterologous antigens. rMVAs encoding proteins of Bluetongue virus (BTV), an orbivirus that infects domestic and wild ruminants through transmission by biting midges of the Culicoides species, are excellent vaccine candidates against this virus. In this chapter, we describe the methods for the generation of rMVAs encoding VP2, NS1, and VP7 proteins of BTV . The included protocols cover the cloning of VP2, NS1, and VP7 BTV-4 genes in a transfer plasmid, the construction of rMVAs, the titration of virus working stocks, and the protein expression analysis by immunofluorescence and radiolabeling of rMVA infected cells as well as virus purification procedure., (© 2022. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2022

4. Recombinant Rift Valley fever viruses encoding bluetongue virus (BTV) antigens: Immunity and efficacy studies upon a BTV-4 challenge.

Author

Moreno S, Calvo-Pinilla E, Devignot S, Weber F, Ortego J, and Brun A

Subjects

Animals, Bluetongue virology, Bluetongue virus genetics, Capsid Proteins genetics, Capsid Proteins immunology, Female, Immunity, Mice, Reassortant Viruses, Rift Valley Fever virology, Rift Valley fever virus genetics, Serogroup, Sheep, Vaccines, Attenuated immunology, Viral Nonstructural Proteins genetics, Viral Nonstructural Proteins immunology, Antibodies, Viral immunology, Antigens, Viral immunology, Bluetongue prevention & control, Bluetongue virus immunology, Rift Valley Fever prevention & control, Vaccination veterinary, Viral Vaccines immunology

Abstract

Background: Many ruminant diseases of viral aetiology can be effectively prevented using appropriate vaccination measures. For diseases such as Rift Valley fever (RVF) the long inter-epizootic periods make routine vaccination programs unfeasible. Coupling RVF prophylaxis with seasonal vaccination programmes by means of multivalent vaccine platforms would help to reduce the risk of new RVF outbreaks., Methodology/principal Findings: In this work we generated recombinant attenuated Rift Valley fever viruses (RVFVs) encoding in place of the virulence factor NSs either the VP2 capsid protein or a truncated form of the non-structural NS1 protein of bluetongue virus serotype 4 (BTV-4). The recombinant viruses were able to carry and express the heterologous BTV genes upon consecutive passages in cell cultures. In murine models, a single immunization was sufficient to protect mice upon RVFV challenge and to elicit a specific immune response against BTV-4 antigens that was fully protective after a BTV-4 boost. In sheep, a natural host for RVFV and BTV, both vaccines proved immunogenic although conferred only partial protection after a virulent BTV-4 reassortant Morocco strain challenge., Conclusions/significance: Though additional optimization will be needed to improve the efficacy data against BTV in sheep, our findings warrant further developments of attenuated RVFV as a dual vaccine platform carrying heterologous immune relevant antigens for ruminant diseases in RVF risk areas., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

5. Microspheres-prime/rMVA-boost vaccination enhances humoral and cellular immune response in IFNAR(-/-) mice conferring protection against serotypes 1 and 4 of bluetongue virus.

Author

Marín-López A, Calvo-Pinilla E, Barriales D, Lorenzo G, Benavente J, Brun A, Martínez-Costas JM, and Ortego J

Subjects

Animals, Antibodies, Neutralizing, Bluetongue virus classification, CD8-Positive T-Lymphocytes metabolism, Capsid Proteins genetics, Capsid Proteins immunology, Cell Line, Chlorocebus aethiops, Immunization, Immunization, Secondary methods, Immunoglobulin G blood, Lysosomal-Associated Membrane Protein 1 metabolism, Male, Mice, Mice, 129 Strain, Orthoreovirus, Avian genetics, Orthoreovirus, Avian immunology, Serogroup, Vaccines, Attenuated immunology, Vaccines, Inactivated immunology, Vaccines, Synthetic immunology, Vero Cells, Viral Core Proteins genetics, Viral Core Proteins immunology, Viral Nonstructural Proteins genetics, Viral Nonstructural Proteins immunology, Viral Vaccines immunology, Bluetongue prevention & control, Bluetongue virus immunology, Immunity, Cellular immunology, Immunity, Humoral immunology, Microspheres, Receptor, Interferon alpha-beta immunology, Vaccination, Vaccinia virus immunology

Abstract

Bluetongue virus (BTV) is the causative agent of bluetongue disease (BT), which affects domestic and wild ruminants. At the present, 27 different serotypes have been documented. Vaccination has been demonstrated as one of the most effective methods to avoid viral dissemination. To overcome the drawbacks associated with the use of inactivated and attenuated vaccines we engineered a new recombinant BTV vaccine candidate based on proteins VP2, VP7, and NS1 of BTV-4 that were incorporated into avian reovirus muNS-Mi microspheres (MS-VP2/VP7/NS1) and recombinant modified vaccinia virus Ankara (rMVA). The combination of these two antigen delivery systems in a heterologous prime-boost vaccination strategy generated significant levels of neutralizing antibodies in IFNAR(-/-) mice. Furthermore, this immunization strategy increased the ratio of IgG2a/IgG1 in sera, indicating an induction of a Th1 response, and elicited a CD8 T cell response. Immunized mice were protected against lethal challenges with the homologous serotype 4 and the heterologous serotype 1 of BTV. All these results support the strategy based on microspheres in combination with rMVAs as a promising multiserotype vaccine candidate against BTV., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

6. Pathological Characterization Of IFNAR(-/-) Mice Infected With Bluetongue Virus Serotype 4.

Author

Marín-López A, Bermúdez R, Calvo-Pinilla E, Moreno S, Brun A, and Ortego J

Subjects

Animals, Bluetongue genetics, Bluetongue virology, Immunohistochemistry, Interleukin-12 metabolism, Interleukin-1beta metabolism, Interleukin-6 metabolism, Leukocytes metabolism, Male, Mice, Receptor, Interferon alpha-beta genetics, Reverse Transcriptase Polymerase Chain Reaction, Serogroup, Tumor Necrosis Factor-alpha metabolism, Bluetongue metabolism, Bluetongue virus pathogenicity, Receptor, Interferon alpha-beta metabolism

Abstract

Bluetongue virus (BTV) replicates in lymphoid tissues where infected mononuclear leukocytes secrete proinflammatory and vasoactive mediators that can contribute to bluetongue (BT) pathogenesis. Using the well-characterized IFNAR(-/-) mice animal model, we have now studied the histopathology and dynamics of leukocyte populations in different target tissues (spleen, thymus, and lung) during BTV-4 infection by histological and immunohistochemical techniques. The spleen and thymus of BTV-4 infected mice showed severe lymphoid depletion on H&E stained sections. This finding was confirmed by IHC, showing moderate decreased immunopositivity against CD3 in the thymus, and scarce immunoreactivity against CD3 and CD79 in the rest of the white pulp in the spleen, together with an increase in MAC387 immunostaining. BTV-4 infection also induced the expression of active caspase-3 in the spleen, where apoptotic debris was observed by H&E. A dramatic increase in iNOS immunoreactivity associated to necrotic areas of the white pulp was observed, being less noticeable in the thymus and the lung. The induction of pro-inflammatory cytokines in tissues where BTV replicates was evaluated by measuring transcript levels by RT-qPCR. BTV-4 infection led to enhance transcription of IFN-γ, TNF, IL-6, IL-12-p40, and IL-1β mRNA in the thymus, spleen and lung, correlating with the level of virus replication in these tissues. Disease progression and pathogenesis in IFNAR(-/-) mice closely mimics hallmarks of bluetongue disease in ruminants. IFNAR(-/-) mice are a good choice to facilitate a faster advance in the field of orbiviruses., Competing Interests: The authors have declared that no competing interest exists.

Published

2016

7. An experimental subunit vaccine based on Bluetongue virus 4 VP2 protein fused to an antigen-presenting cells single chain antibody elicits cellular and humoral immune responses in cattle, guinea pigs and IFNAR(-/-) mice.

Author

Legisa DM, Perez Aguirreburualde MS, Gonzalez FN, Marin-Lopez A, Ruiz V, Wigdorovitz A, Martinez-Escribano JA, Ortego J, and Dus Santos MJ

Subjects

Animals, Antibodies, Neutralizing blood, Antibodies, Viral blood, Baculoviridae genetics, Capsid Proteins administration & dosage, Cattle, Female, Guinea Pigs, Immunity, Cellular, Immunity, Humoral, Mice, Mice, Knockout, Recombinant Proteins, Vaccination, Vaccines, Subunit administration & dosage, Vaccines, Synthetic administration & dosage, Vaccines, Synthetic immunology, Antigen-Presenting Cells immunology, Bluetongue prevention & control, Bluetongue virus immunology, Capsid Proteins immunology, Receptor, Interferon alpha-beta genetics, Vaccines, Subunit immunology

Abstract

Bluetongue virus (BTV), the causative agent of bluetongue disease (BT) in domestic and wild ruminants, is worldwide distributed. A total of 27 serotypes have been described so far, and several outbreaks have been reported. Vaccination is critical for controlling the spread of BTV. In the last years, subunit vaccines, viral vector vaccines and reverse genetic-based vaccines have emerged as new alternatives to conventional ones. In this study, we developed an experimental subunit vaccine against BTV4, with the benefit of targeting the recombinant protein to antigen-presenting cells. The VP2 protein from an Argentine BTV4 isolate was expressed alone or fused to the antigen presenting cell homing (APCH) molecule, in the baculovirus insect cell expression system. The immunogenicity of both proteins was evaluated in guinea pigs and cattle. Titers of specific neutralizing antibodies in guinea pigs and cattle immunized with VP2 or APCH-VP2 were high and similar to those induced by a conventional inactivated vaccine. The immunogenicity of recombinant proteins was further studied in the IFNAR(-/-) mouse model where the fusion of VP2 to APCH enhanced the cellular immune response and the neutralizing activity induced by VP2., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

8. Interferon α/β receptor knockout mice as a model to study bluetongue virus infection.

Author

Ortego J, de la Poza F, and Marín-López A

Subjects

Animals, Bluetongue immunology, Bluetongue prevention & control, Bluetongue virus pathogenicity, Mice, Mice, Knockout, Viral Vaccines administration & dosage, Viral Vaccines immunology, Bluetongue pathology, Bluetongue virology, Bluetongue virus immunology, Bluetongue virus physiology, Disease Models, Animal, Receptor, Interferon alpha-beta deficiency

Abstract

Bluetongue is an arthropod-borne disease caused by a virus of the genus Orbivirus, the bluetongue virus (BTV), which affects ruminant livestock such as cattle, sheep, and goats and wild ruminants such as deer, and camelids. Recently, adult mice with gene knockouts of the interferon α/β receptor (IFNAR-/-) have been described as a model of lethal BTV infection. IFNAR(-/-) mice are highly susceptible to BTV-1, BTV-4 and BTV-8 infection when the virus is administered intravenously or subcutaneosuly. Disease progression and pathogenesis closely mimics signs of bluetongue disease in ruminants. In the present paper we review the studies where IFNAR(-/-) mice have been used as an animal model to study BTV transmission, pathogenesis, virulence, and protective efficacy of inactivated and new recombinant marker BTV vaccines. Furthermore, we report new data on protective efficacy of different strategies of BTV vaccination and also on induction of interferon α/β and proinflammatory immune responses in IFNAR(-/-) mice infected with BTV., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2014

9. Recombinant vaccines against bluetongue virus.

Author

Calvo-Pinilla E, Castillo-Olivares J, Jabbar T, Ortego J, de la Poza F, and Marín-López A

Subjects

Animals, Bluetongue epidemiology, Communicable Diseases, Emerging epidemiology, Communicable Diseases, Emerging prevention & control, Europe epidemiology, Vaccines, Synthetic genetics, Vaccines, Synthetic immunology, Vaccines, Synthetic isolation & purification, Viral Vaccines genetics, Bluetongue prevention & control, Bluetongue virus immunology, Communicable Diseases, Emerging veterinary, Viral Vaccines immunology, Viral Vaccines isolation & purification

Abstract

Bluetongue (BT) is a hemorrhagic disease of ruminants caused by bluetongue virus (BTV), the prototype member of the genus Orbivirus within the family Reoviridae and is transmitted via biting midges of the genus Culicoides. BTV can be found on all continents except Antarctica, and up to 26 immunologically distinct BTV serotypes have been identified. Live attenuated and inactivated BTV vaccines have been used over the years with different degrees of success. The multiple outbreaks of BTV in Mediterranean Europe in the last two decades and the incursion of BTV-8 in Northern Europe in 2008 has re-stimulated the interest to develop improved vaccination strategies against BTV. In particular, safer, cross-reactive, more efficacious vaccines with differential diagnostic capability have been pursued by multiple BTV research groups and vaccine manufacturers. A wide variety of recombinant BTV vaccine prototypes have been investigated, ranging from baculovirus-expressed sub-unit vaccines to the use of live viral vectors. This article gives a brief overview of all these modern approaches to develop vaccines against BTV including some recent unpublished data., (Copyright © 2013 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2014

10. Protection of IFNAR (-/-) mice against bluetongue virus serotype 8, by heterologous (DNA/rMVA) and homologous (rMVA/rMVA) vaccination, expressing outer-capsid protein VP2.

Author

Jabbar TK, Calvo-Pinilla E, Mateos F, Gubbins S, Bin-Tarif A, Bachanek-Bankowska K, Alpar O, Ortego J, Takamatsu HH, Mertens PP, and Castillo-Olivares J

Subjects

Animals, Antibodies, Neutralizing blood, Bluetongue blood, Bluetongue virology, Chickens, Chlorocebus aethiops, Mice, Plasmids immunology, RNA, Viral blood, Receptor, Interferon alpha-beta metabolism, Vaccination, Vero Cells, Viremia immunology, Viremia prevention & control, Viremia virology, Bluetongue immunology, Bluetongue prevention & control, Bluetongue virus immunology, Capsid Proteins immunology, Receptor, Interferon alpha-beta deficiency, Vaccines, DNA immunology, Vaccines, Synthetic immunology

Abstract

The protective efficacy of recombinant vaccines expressing serotype 8 bluetongue virus (BTV-8) capsid proteins was tested in a mouse model. The recombinant vaccines comprised plasmid DNA or Modified Vaccinia Ankara viruses encoding BTV VP2, VP5 or VP7 proteins. These constructs were administered alone or in combination using either a homologous prime boost vaccination regime (rMVA/rMVA) or a heterologous vaccination regime (DNA/rMVA). The DNA/rMVA or rMVA/rMVA prime-boost were administered at a three week interval and all of the animals that received VP2 generated neutralising antibodies. The vaccinated and non-vaccinated-control mice were subsequently challenged with a lethal dose of BTV-8. Mice vaccinated with VP7 alone were not protected. However, mice vaccinated with DNA/rMVA or rMVA/rMVA expressing VP2, VP5 and VP7 or VP2 alone were all protected.

Published

2013

11. Immunization of knock-out α/β interferon receptor mice against lethal bluetongue infection with a BoHV-4-based vector expressing BTV-8 VP2 antigen.

Author

Franceschi V, Capocefalo A, Calvo-Pinilla E, Redaelli M, Mucignat-Caretta C, Mertens P, Ortego J, and Donofrio G

Subjects

Amino Acid Sequence, Animals, Antibodies, Neutralizing, Antibodies, Viral blood, Base Sequence, Bluetongue immunology, Bluetongue virus immunology, Capsid Proteins genetics, Cattle, Cell Line, Chlorocebus aethiops, Cricetinae, Dogs, Genetic Vectors, Herpesvirus 4, Bovine immunology, Humans, Male, Mice, Mice, Knockout, Molecular Sequence Data, Pilot Projects, Viral Plaque Assay, Viral Vaccines genetics, Viremia immunology, Bluetongue prevention & control, Capsid Proteins immunology, Receptor, Interferon alpha-beta genetics, Viral Vaccines immunology

Abstract

New effective tools for vaccine strategies are necessary to limit the spread of bluetongue, an insect-transmitted viral disease of domestic and wild ruminants. In the present study, BoHV-4-based vector cloned as a bacterial artificial chromosome (BAC) was engineered to express the bluetongue virus (BTV) immune-dominant glycoprotein VP2 provided of a heterologous signal peptide to its amino terminal and a trans-membrane domain to its carboxyl terminal (IgK-VP2gDtm), to allow the VP2 expression targeting to the cell membrane fraction. Based on adult α/β interferon receptor knockout (IFNAR(-/-)) mice, a newly generated bluetongue laboratory animal model, a pre-challenge experiment was performed to test BoHV-4 safety on such immune-compromised animal. BoHV-4 infected IFNAR(-/-) mice did not show clinical signs even following the inoculation of BoHV-4 intra-cerebrally, although many areas of the brain got transduced. IFNAR(-/-) mice intraperitoneally inoculated twice with BoHV-4-A-IgK-VP2gDtm at different time points developed serum neutralizing antibodies against BTV and showed a strongly reduced viremia and a longer survival time when challenged with a lethal dose of BTV-8. The data acquired in this pilot study validate BoHV-4-based vector as a safe and effective heterologous antigen carrier/producer for the formulation of enhanced recombinant immunogens for the vaccination against lethal bluetongue., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published

2011

12. Experimental oral infection of bluetongue virus serotype 8 in type I interferon receptor-deficient mice.

Author

Calvo-Pinilla E, Nieto JM, and Ortego J

Subjects

Animal Structures pathology, Animal Structures virology, Animals, Female, Histocytochemistry, Male, Mice, Microscopy, Sheep, Survival Analysis, Viral Load, Viremia, Bluetongue pathology, Bluetongue virology, Bluetongue virus pathogenicity, Disease Models, Animal, Receptor, Interferon alpha-beta deficiency

Abstract

The identification of transmission routes for bluetongue virus (BTV) is essential to improve the control of the disease. Although BTV is primarily transmitted by several species of Culicoides biting midges, there has been evidence of transplacental and oral transmission. We now report that IFNAR((-/-)) mice are susceptible to oral infection by BTV-8. Viraemia, clinical manifestations and tissue lesions are similar to those in intravenously infected mice. In addition, we show that the oral cavity and oesophagus are susceptible to BTV infection and replication, suggesting that these organs are possible entry routes during BTV oral infection.

Published

2010

13. Heterologous prime boost vaccination with DNA and recombinant modified vaccinia virus Ankara protects IFNAR(-/-) mice against lethal bluetongue infection.

Author

Calvo-Pinilla E, Rodríguez-Calvo T, Sevilla N, and Ortego J

Subjects

Animals, Bluetongue virus metabolism, Capsid Proteins genetics, Cell Line, Chickens, Chlorocebus aethiops, Cricetinae, Mice, Vero Cells, Bluetongue immunology, Bluetongue prevention & control, Bluetongue virus immunology, Capsid Proteins immunology, Vaccination methods, Vaccines, DNA immunology, Vaccinia virus immunology

Abstract

Recent recombinant DNA technology has provided novel approaches to develop marker and safe vaccines against bluetongue virus (BTV). To develop new vaccination strategies against BTV infection we have engineered naked DNAs and recombinant modified vaccinia virus Ankara (rMVA) expressing VP2, VP5 and VP7 proteins from BTV-4. IFNAR(-/-) mice inoculated with DNA/rMVA-VP2, -VP5, -VP7 in an heterologous prime boost vaccination strategy generated significant levels of neutralizing antibodies against BTV-4 and they were completely protected against BTV-4 challenge. Interestingly, VP2 and VP7 proteins expressed in the DNA/rMVA vaccines induced a specific BTV T-cell response that might contribute to the protection of IFNAR(-/-) mice against challenge with BTV-4. In addition, antibodies against VP2, VP5, and VP7, but not NS3 were detected in the sera of DNA/rMVA-VP2, -VP5, -VP7 immunized mice confirming the DIVA (differentiating infected from vaccinated animals) properties of this vaccine. Overall, our results show that the heterologous prime boost vaccination with DNA/rMVA expressing VP2, VP5, and VP7 proteins protects against BTV-4 infection.

Published

2009

14. Establishment of a bluetongue virus infection model in mice that are deficient in the alpha/beta interferon receptor.

Author

Calvo-Pinilla E, Rodríguez-Calvo T, Anguita J, Sevilla N, and Ortego J

Subjects

Animals, Bluetongue prevention & control, Bluetongue virus genetics, Bluetongue virus pathogenicity, Cell Line, Lung pathology, Lung virology, Lymph Nodes pathology, Lymph Nodes virology, Mice, Mice, Inbred C57BL, Mice, Knockout, Spleen pathology, Spleen virology, Survival Rate, Viral Vaccines immunology, Bluetongue immunology, Bluetongue virus immunology, Receptor, Interferon alpha-beta genetics, Receptor, Interferon alpha-beta immunology

Abstract

Bluetongue (BT) is a noncontagious, insect-transmitted disease of ruminants caused by the bluetongue virus (BTV). A laboratory animal model would greatly facilitate the studies of pathogenesis, immune response and vaccination against BTV. Herein, we show that adult mice deficient in type I IFN receptor (IFNAR((-/-))) are highly susceptible to BTV-4 and BTV-8 infection when the virus is administered intravenously. Disease was characterized by ocular discharges and apathy, starting at 48 hours post-infection and quickly leading to animal death within 60 hours of inoculation. Infectious virus was recovered from the spleen, lung, thymus, and lymph nodes indicating a systemic infection. In addition, a lymphoid depletion in spleen, and severe pneumonia were observed in the infected mice. Furthermore, IFNAR((-/-)) adult mice immunized with a BTV-4 inactivated vaccine showed the induction of neutralizing antibodies against BTV-4 and complete protection against challenge with a lethal dose of this virus. The data indicate that this mouse model may facilitate the study of BTV pathogenesis, and the development of new effective vaccines for BTV.

Published

2009