Your search keyword '"Lorraine Frost"' showing total 13 results

1. Outbreak of African horse sickness in Thailand, 2020

Author

Simon Carpenter, Carrie Batten, Simon King, Paulina Rajko-Nenow, Martin Ashby, and Lorraine Frost

Subjects

Serotype, 0303 health sciences, General Veterinary, General Immunology and Microbiology, biology, 040301 veterinary sciences, Incidence (epidemiology), Outbreak, 04 agricultural and veterinary sciences, General Medicine, biology.organism_classification, 0403 veterinary science, 03 medical and health sciences, Geography, parasitic diseases, African horse sickness, South east asia, Socioeconomics, 030304 developmental biology

Abstract

African horse sickness was confirmed in horses in Thailand during March 2020. The virus was determined to belong to serotype 1 and is phylogenetically closely related to isolates from South Africa. This is the first incidence of African horse sickness occurring in South East Asia and of serotype 1 outside of Africa.

Published

2020

2. Complete Coding Sequence of a Novel Bluetongue Virus Isolated from a Commercial Sheeppox Vaccine

Author

Hannah M. Brown, John Flannery, Paulina Rajko-Nenow, Velizar Bumbarov, Lorraine Frost, Karin E. Darpel, Carrie Batten, Chandana Tennakoon, and Natalia Golender

Subjects

0301 basic medicine, Sheeppox, Strain (chemistry), 040301 veterinary sciences, Genome Sequences, 04 agricultural and veterinary sciences, Biology, Virology, Genome, Sequence identity, Virus, 3. Good health, 0403 veterinary science, 03 medical and health sciences, 030104 developmental biology, Immunology and Microbiology (miscellaneous), Genotype, Genetics, Coding region, Molecular Biology

Abstract

The full genome sequences of two isolates of bluetongue virus (BTV) from a commercial sheeppox vaccine were determined. Strain SPvvvv/02 shows low sequence identity to its closest relative, strain BTV-26 KUW2010/02, indicating the probable detection of a novel BTV genotype, whereas strain SPvvvv/03 shows high sequence identity to strain BTV-28/1537/14.

Published

2020

3. BTV-14 Infection in Sheep Elicits Viraemia with Mild Clinical Symptoms

Author

Petra C. Fay, Hayley Hicks, Marcin Smreczak, Lorraine Frost, Anna Orłowska, Paulina Rajko-Nenow, Karin E. Darpel, Carrie Batten, Mark Henstock, and John Flannery

Subjects

0301 basic medicine, Microbiology (medical), Conjunctiva, 040301 veterinary sciences, real-time RT-PCR, Microbiology, Asymptomatic, Arbovirus, 0403 veterinary science, 03 medical and health sciences, Vaccine strain, Virology, medicine, Bluetongue virus serotype, lcsh:QH301-705.5, bluetongue, biology, business.industry, Brief Report, virus diseases, 04 agricultural and veterinary sciences, medicine.disease, arbovirus, 030104 developmental biology, medicine.anatomical_structure, Dorset sheep, lcsh:Biology (General), biology.protein, infection kinetics, medicine.symptom, Antibody, business, Sheep breed

Abstract

In 2011, Bluetongue virus serotype 14 (BTV-14) was detected in Russia during routine surveillance, and was subsequently found in a number of European countries. The strain had high sequence similarity to a BTV-14 vaccine strain. We aimed to determine the risk of this BTV-14 strain causing disease in a UK sheep breed. Four Poll Dorset sheep were infected with a Polish isolate of BTV-14 and infection kinetics were monitored over 28 days. BTV RNA was detected in EDTA blood by 4 days post-infection (dpi) and remained detectable at 28 days post-infection (dpi). Peak viraemia occurred at 6 and 7 dpi with Ct values ranging between 24.6 and 27.3 in all infected animals. BTV antibodies were detected by 10 dpi using a commercial ELISA and neutralising antibodies were detected from 10 dpi. BTV was isolated between 6 and 12 dpi. All infected sheep developed mild clinical signs such as reddening of conjunctiva and mucosal membranes, with one sheep demonstrating more overt clinical signs. Two uninoculated control animals remained clinically healthy and did not have detectable BTV RNA or antibodies. The overall mild clinical symptoms caused by this BTV-14 in this highly susceptible sheep breed were in accordance with the asymptomatic infections observed in the affected countries.

Published

2020

4. Evidence of reduced viremia, pathogenicity and vector competence in a re-emerging European strain of bluetongue virus serotype 8 in sheep

Author

Christopher Sanders, Simon Gubbins, Lyndsay Cooke, Paulina Rajko-Nenow, Simon Carpenter, Martin Ashby, Hannah M. Brown, Matthew Tully, Emmanuel Bréard, John Flannery, Hayley Hicks, Beatriz Sanz-Bernardo, Amanda Corla, Corinne Sailleau, Mehnaz Qureshi, Stéphan Zientara, Carrie Batten, Lorraine Frost, Karin E. Darpel, Pirbright Institute, Virologie UMR1161 (VIRO), Institut National de la Recherche Agronomique (INRA)-Agence nationale de sécurité sanitaire de l'alimentation, de l'environnement et du travail (ANSES)-École nationale vétérinaire d'Alfort (ENVA), Université Paris Est, European CommissionEuropean Commission Joint Research Centre, Department for Environment, Food and Rural Affairs (Defra)Department for Environment, Food & Rural Affairs (DEFRA) [SE2621], and Biotechnology and Biological Sciences Research Council (BBSRC)Biotechnology and Biological Sciences Research Council (BBSRC) [BBS/E/I/00007030, BBS/E/I/00007033, BBS/E/I/00007036, BBS/E/I/00007037]

Subjects

Serotype, European serotypes, virus isolation RT-qPCR, 040301 veterinary sciences, [SDV]Life Sciences [q-bio], Viremia, Antibodies, Viral, Ceratopogonidae, Serogroup, Bluetongue, Communicable Diseases, Emerging, virus isolation RT‐qPCR, Virus, Disease Outbreaks, 0403 veterinary science, 03 medical and health sciences, bluetongue virus, Bluetongue disease, medicine, Animals, 030304 developmental biology, 2. Zero hunger, 0303 health sciences, Sheep, Virulence, General Veterinary, General Immunology and Microbiology, biology, Inoculation, business.industry, Outbreak, Original Articles, General Medicine, 04 agricultural and veterinary sciences, medicine.disease, Virology, Insect Vectors, Lameness, arboviruses, biology.protein, Female, Original Article, Livestock, France, infection kinetics, Antibody, business

Abstract

SummaryThe outbreak of bluetongue virus (BTV) serotype 8 (BTV-8) during 2006-2009 in Europe was the most costly epidemic of the virus in recorded history. In 2015, a BTV-8 strain re-emerged in France which has continued to circulate since then. To examine anecdotal reports of reduced pathogenicity and transmission efficiency, we investigated the infection kinetics of a 2007 UK BTV-8 strain alongside the re-emerging BTV-8 strain isolated from France in 2017. Two groups of eight BTV-naïve British mule sheep were inoculated with 5.75 log10TCID50 ml−1 of either BTV-8 strain. BTV RNA was detected by 2 dpi in both groups with peak viremia occurring between 5-9 dpi. A significantly greater amount of BTV RNA was detected in sheep infected with the 2007 strain (6.0-8.8 log10 genome copies mL−1) than the re-emerging BTV-8 strain (2.9-7.9 log10 genome copies mL−1). All infected sheep developed BTV-specific antibodies by 9 dpi. BTV was isolated from 2 dpi to 12 dpi for 2007 BTV-8-inoculated sheep and from 5 to 10 dpi for sheep inoculated with the remerging BTV-8. In Culicoides sonorensis feeding on the sheep over the period 7-12 dpi, vector competence was significantly higher for the 2007 strain than the re-emerging strain. Both the proportion of animals showing moderate (as opposed to mild or no) clinical disease (6/8 vs 1/8) and the overall clinical scores (median 5.25 vs 3) were significantly higher in sheep infected with the 2007 strain, compared to those infected with the re-emerging strain. However, one sheep infected with the re-emerging strain was euthanized at 16 dpi having developed severe lameness. This highlights the potential of the re-emerging BTV-8 to still cause illness in naïve ruminants with concurrent costs to the livestock industry.SummaryThe re-emerging Bluetongue virus serotype 8 still presents a threat to naïve ruminants in Europe despite reduced virulence

Published

2019

5. Assessment of reproducibility of a VP7 Blocking ELISA diagnostic test for african horse sickness

Author

Paloma Rueda, Stéphan Zientara, Sylvie Lecollinet, Cristina Tena-Tomás, Christiaan A. Potgieter, Manuel Durán‐Ferrer, Baratang Alison Lubisi, Tracy Sturgill, Eileen N. Ostlund, Carrie Batten, Simon Gubbins, Corinne Sailleau, Lorraine Frost, John Flannery, José Manuel Sánchez-Vizcaíno, Patricia Sastre, Montserrat Agüero, Ruben Villalba, Javier Castillo-Olivares, Shirley Jacqueline Smith, Federica Monaco, Cécile Beck, Michelle Emery, LCV, Partenaires INRAE, Virologie UMR1161 (VIRO), École nationale vétérinaire d'Alfort (ENVA)-Institut National de la Recherche Agronomique (INRA)-Agence nationale de sécurité sanitaire de l'alimentation, de l'environnement et du travail (ANSES), North West University, INGENASA, IZS Abruzzo & Molise, Teramo, Italy, Pirbright Institute, Onderstepoort Veterinary Institute, ARC, Universidad Complutense de Madrid = Complutense University of Madrid [Madrid] (UCM), United States Department of Agriculture (USDA), World Organisation of Animal Health (OIE) [AD/SR/2015/1885], Biotechnology and Biological Sciences Research Council [BBS/E/I/00002536, BBS/E/I/00007036, BBS/E/I/00007037], Castillo-Olivares, Javier, and 10085637 - Potgieter, Abraham Christiaan

Subjects

[SDV]Life Sciences [q-bio], Blocking (statistics), Serology, 0403 veterinary science, Epidemiology, Medicine, antibodies, diagnostic sensitivity, Antigens, Viral, 0303 health sciences, education.field_of_study, biology, Viral Core Proteins, Ring trial, Diagnostic test, 04 agricultural and veterinary sciences, General Medicine, performance characteristics, Reproducibility, 3. Good health, African horse sickness, ring trial, Original Article, ELISA, medicine.medical_specialty, 040301 veterinary sciences, Population, Enzyme-Linked Immunosorbent Assay, Antibodies, 03 medical and health sciences, Diagnostic specificity, Internal medicine, African Horse Sickness Virus, Animals, Horses, education, reproducibility, 030304 developmental biology, Immune status, General Veterinary, General Immunology and Microbiology, business.industry, Diagnostic Tests, Routine, Programme implementation, Reproducibility of Results, Original Articles, biology.organism_classification, Performance characteristics, Diagnostic sensitivity, diagnostic specificity, Horse Diseases, business

Abstract

International audience; The laboratory diagnosis of African horse sickness (AHS) is important for: (a) demonstrating freedom from infection in a population, animals or products for trade (b) assessing the efficiency of eradication policies; (c) laboratory confirmation of clinical diagnosis; (d) estimating the prevalence of AHS infection; and (e) assessing postvaccination immune status of individual animals or populations. Although serological techniques play a secondary role in the confirmation of clinical cases, their use is very important for all the other purposes due to their high throughput, ease of use and good cost-benefit ratio. The main objective of this study was to support the validation of AHS VP7 Blocking ELISA up to the Stage 3 of the World Animal Health Organization (OIE) assay validation pathway. To achieve this, a collaborative ring trial, which included all OIE Reference Laboratories and other AHS-specialist diagnostic centres, was conducted in order to assess the diagnostic performance characteristics of the VP7 Blocking ELISA. In this trial, a panel of sera of different epidemiological origin and infection status was used. Through this comprehensive evaluation we can conclude that the VP7 Blocking ELISA satisfies the OIE requirements of reproducibility. The VP7 Blocking ELISA, in its commercial version is ready to enter Stage 4 of the validation pathway (Programme Implementation). Specifically, this will require testing the diagnostic performance of the assay using contemporary serum samples collected during control campaigns in endemic countries.

Published

2019

6. Bluetongue virus infection in naïve cattle: Identification of circulating serotypes and associated Culicoides biting midge species in Trinidad

Author

R. Ramdeen, Tamiko Brown-Joseph, John Flannery, Vernie Ramkissoon, Lara E. Harrup, Lorraine Frost, Carrie Batten, Christine V.F. Carrington, Hayley Hicks, and Christopher A. L. Oura

Subjects

0301 basic medicine, Serotype, Male, Veterinary medicine, 040301 veterinary sciences, Virus isolation, viruses, Biting midge, Cattle Diseases, Biology, Antibodies, Viral, Ceratopogonidae, Serogroup, Microbiology, Bluetongue, Virus, Article, Serology, 0403 veterinary science, 03 medical and health sciences, Animals, 2. Zero hunger, General Veterinary, business.industry, virus diseases, 04 agricultural and veterinary sciences, General Medicine, Virology, 3. Good health, Insect Vectors, 030104 developmental biology, Trinidad and Tobago, Livestock, Cattle, Female, business, Bluetongue virus

Abstract

Highlights • High prevalence of bluetongue virus in Trinidad. • Identification of six bluetongue virus serotypes in Trinidad. • First isolation of BTV-2 and BTV-5 in Trinidad. • Risk of emergence of reassortant viruses., To better understand risks associated with trading cattle, it is important to know which serotypes of Bluetongue virus (BTV) are circulating within the exporting and importing country. Hence, this study was conducted to identify the circulating serotypes of BTV in Trinidad. Blood samples were collected monthly from sixty BTV- naïve imported cattle over a six month period after their arrival in the country. Virological (PCR and virus isolation) and serological (ELISA) analyses were carried out on the samples and CDC light traps were placed near the cattle enclosure to trap and identify the species of Culicoides biting midges that were present. All of the cattle seroconverted for BTV antibodies within three months of their arrival in the country and real-time reverse transcription PCR (rRT-PCR) detected BTV-RNA in the samples throughout the remainder of the study. The patterns of infection observed in the cattle indicated serial infections with multiple serotypes. A combination of BTV serotype-specific rRT-PCR on the original blood samples and virus isolation followed by serotype-specific rRT-PCR on selected samples, confirmed the presence of BTV serotypes 1, 2, 3, 5, 12 and 17. This is the first report of BTV-2 and BTV-5 in Trinidad. Light-suction traps placed in close proximity to the cattle predominantly trapped Culicoides insignis Lutz 1913 species (96%), with a further six Culicoides species making up the remaining 4% of trapped samples. The circulation of multiple BTV serotypes in Trinidad underlines the need for regular surveillance, which will contribute to the development of risk assessments for trade in livestock.

Published

2017

7. Peste des Petits Ruminants Infection among Cattle and Wildlife in Northern Tanzania

Author

Lorraine Frost, C.A.L. Oura, Carrie Batten, Robert D. Fyumagwa, Fredrick M. Kivaria, Chobi Chubwa, Tiziana Lembo, Richard Kock, Sarah Cleaveland, Richard Hoare, and Satya Parida

Subjects

Microbiology (medical), Veterinary medicine, 040301 veterinary sciences, Epidemiology, wildlife, Spillover infection, Wildlife, Cattle Diseases, lcsh:Medicine, Animals, Wild, Antibodies, Viral, Tanzania, Rinderpest, Peste-des-petits-ruminants virus, lcsh:Infectious and parasitic diseases, 0403 veterinary science, 03 medical and health sciences, Seroepidemiologic Studies, Peste-des-Petits-Ruminants, Animals, viruses, lcsh:RC109-216, Geography, Medical, Serotyping, 030304 developmental biology, 2. Zero hunger, 0303 health sciences, biology, lcsh:R, Dispatch, Outbreak, 04 agricultural and veterinary sciences, biology.organism_classification, peste des petits ruminants, morbillivirus, Infectious Diseases, serosurveillance, cattle, disease eradication, rinderpest

Abstract

We investigated peste des petits ruminants (PPR) infection in cattle and wildlife in northern Tanzania. No wildlife from protected ecosystems were seropositive. However, cattle from villages where an outbreak had occurred among small ruminants showed high PPR seropositivity, indicating that spillover infection affects cattle. Thus, cattle could be of value for PPR serosurveillance.

Published

2013

8. Using shared needles for subcutaneous inoculation can transmit bluetongue virus mechanically between ruminant hosts

Author

Karin E. Darpel, Lorraine Frost, Mark Henstock, Eva Veronesi, Andrew Hope, Anthony J. Wilson, Peter P. C. Mertens, Simon Carpenter, C.A.L. Oura, James Barber, Simon Gubbins, Carrie Batten, Katy Moffat, Philip S. Mellor, University of Zurich, and Darpel, Karin E

Subjects

10078 Institute of Parasitology, 0301 basic medicine, Veterinary medicine, Injections, Intradermal, 040301 veterinary sciences, 610 Medicine & health, Infusions, Subcutaneous, Real-Time Polymerase Chain Reaction, qw_806, Arbovirus, Bluetongue, wa_110, Virus, Article, Incubation period, 0403 veterinary science, 03 medical and health sciences, 600 Technology, medicine, Animals, qx_505, Pathogen, Needle sharing, Immunoassay, 1000 Multidisciplinary, Multidisciplinary, Sheep, biology, Transmission (medicine), Inoculation, 04 agricultural and veterinary sciences, Culicoides, biology.organism_classification, medicine.disease, Virology, 3. Good health, 030104 developmental biology, Needles, qw_160, 570 Life sciences, RNA, Viral, Cattle, Bluetongue virus

Abstract

Bluetongue virus (BTV) is an economically important arbovirus of ruminants that is transmitted by Culicoides spp. biting midges. BTV infection of ruminants results in a high viraemia, suggesting that repeated sharing of needles between animals could result in its iatrogenic transmission. Studies defining the risk of iatrogenic transmission of blood-borne pathogens by less invasive routes, such as subcutaneous or intradermal inoculations are rare, even though the sharing of needles is common practice for these inoculation routes in the veterinary sector. Here we demonstrate that BTV can be transmitted by needle sharing during subcutaneous inoculation, despite the absence of visible blood contamination of the needles. The incubation period, measured from sharing of needles, to detection of BTV in the recipient sheep or cattle, was substantially longer than has previously been reported after experimental infection of ruminants by either direct inoculation of virus, or through blood feeding by infected Culicoides. Although such mechanical transmission is most likely rare under field condition, these results are likely to influence future advice given in relation to sharing needles during veterinary vaccination campaigns and will also be of interest for the public health sector considering the risk of pathogen transmission during subcutaneous inoculations with re-used needles.

Published

2016

9. Early changes in cytokine expression in peste des petits ruminants disease

Author

Michael D. Baron, Lorraine Frost, A. Bin-Tarif, Geraldine Taylor, Jana Baron, and Rebecca Herbert

Subjects

Male, 040301 veterinary sciences, [SDV]Life Sciences [q-bio], Disease, Biology, Real-Time Polymerase Chain Reaction, Virus, Peste-des-petits-ruminants virus, 0403 veterinary science, Pathogenesis, 03 medical and health sciences, Peste-des-Petits-Ruminants, Bacteriology, Animals, RNA, Messenger, 030304 developmental biology, 0303 health sciences, Goat Diseases, General Veterinary, Research, Goats, 04 agricultural and veterinary sciences, veterinary(all), Virology, 3. Good health, Interleukin 10, Cytokines, Viral disease

Abstract

International audience; Peste des petits ruminants is a viral disease of sheep and goats that has spread through most of Africa as well as the Middle East and the Indian subcontinent. Although, the spread of the disease and its economic impact has made it a focus of international concern, relatively little is known about the nature of the disease itself. We have studied the early stages of pathogenesis in goats infected with six different isolates of Peste des petits ruminants virus representing all four known lineages of the virus. No lineage-specific difference in the pathogenicity of the virus isolates was observed, although there was evidence that even small numbers of cell culture passages could affect the degree of pathogenicity of an isolate. A consistent reduction in CD4+ T cells was observed at 4 days post infection (dpi). Measurement of the expression of various cytokines showed elements of a classic inflammatory response but also a relatively early induction of interleukin 10, which may be contributing to the observed disease.

Published

2014

10. Real-Time Reverse Transcriptase PCR for the Detection of Bluetongue Virus

Author

Lorraine Frost, C.A.L. Oura, and Carrie Batten

Subjects

Reverse transcription polymerase chain reaction, Diagnostic methods, Biology, Virology, Genome, Virus, Oligonucleotide primers

Abstract

In recent years, real-time reverse transcription polymerase chain reaction (rRT-PCR) has become one of the most widely used methods for the diagnosis of infectious pathogens. The combined properties of high sensitivity, specificity, and speed, along with a low contamination risk, have made real-time PCR technology a highly attractive alternative to more conventional diagnostic methods. Numerous robust rRT-PCR systems have been developed and validated for important epizootic diseases of livestock, and in this chapter we describe an rRT-PCR protocol for the detection of bluetongue virus. The assay uses oligonucleotide primers to specifically amplify target regions of the viral genome and a dual-labeled fluorogenic (TaqMan®) probe which allows for the assay to be performed in a closed-tube format, thus minimizing the potential for cross-contamination.

Published

2014

11. Development and testing of a field diagnostic assay for peste des petits ruminants virus

Author

Muhammad Abubakar, Bryony A. Jones, Jana Baron, E Fishbourne, E Couacy-Hyman, G Van't Klooster, Philip G. Toye, J Bashiruddin, T R Chibssa, M Afzal, Chrisostom Ayebazibwe, Lorraine Frost, Rebecca Herbert, and Michael D. Baron

Subjects

Veterinary medicine, disease control, Immunochromatographic test, Sheep Diseases, Field tests, virus, Biology, emerging diseases, Polymerase Chain Reaction, Sensitivity and Specificity, Virus, law.invention, Peste-des-petits-ruminants virus, law, Peste-des-Petits-Ruminants, diagnostics, Animals, Pakistan, Polymerase chain reaction, Africa South of the Sahara, Goat Diseases, Sheep, General Veterinary, General Immunology and Microbiology, Goats, General Medicine, Virology, Rapid Communications, Disease prevention, Field conditions

Abstract

We have developed an immunochromatographic test for the diagnosis of peste des petits ruminants (PPR) under field conditions. The diagnostic assay has been tested in the laboratory and also under field conditions in Ivory Coast, Pakistan, Ethiopia and Uganda. The test is carried out on a superficial swab sample (ocular or nasal) and showed a sensitivity of 84% relative to PCR. The specificity was 95% over all nasal and ocular samples. The test detected as little as 10(3) TCID50 (50% tissue culture infectious doses) of cell culture-grown virus, and detected virus isolates representing all four known genetic lineages of peste des petits ruminants virus. Virus could be detected in swabs from animals as early as 4 days post-infection, at a time when clinical signs were minimal. Feedback from field trials was uniformly positive, suggesting that this diagnostic tool may be useful for current efforts to control the spread of PPR.

Published

2014

12. Evidence for transmission of bluetongue virus serotype 26 through direct contact

Author

Karin E. Darpel, Mark Henstock, Simon Gubbins, Carrie Batten, Eva Veronesi, C.A.L. Oura, Samantha Graves, Petra C. Fay, and Lorraine Frost

Subjects

Serotype, Veterinary medicine, Ceratopogonidae, Epidemiology, Science, Veterinary Microbiology, Serogroup, Bluetongue, Models, Biological, Microbiology, Virus, Infectious Disease Epidemiology, Veterinary Epidemiology, Virology, Medicine and Health Sciences, Animals, Incubation, Multidisciplinary, biology, Population Biology, Transmission (medicine), Goats, Biology and Life Sciences, Veterinary Virology, Blood meal, Culicoides, biology.organism_classification, Insect Vectors, Viral Disease Diagnosis, Viral replication, Veterinary Diseases, RNA, Viral, Medicine, Veterinary Science, Viral Vectors, Bluetongue virus, Viral Transmission and Infection, Research Article

Abstract

The aim of this study was to assess the mechanisms of transmission of bluetongue virus serotype 26 (BTV-26) in goats. A previous study, which investigated the pathogenicity and infection kinetics of BTV-26 in goats, unexpectedly revealed that one control goat may have been infected through a direct contact transmission route. To investigate the transmission mechanisms of BTV-26 in more detail an experimental infection study was carried out in which three goats were infected with BTV-26, three goats were kept uninfected, but were housed in direct contact with the infected goats, and an additional four goats were kept in indirect contact separated from infected goats by metal gates. This barrier allowed the goats to have occasional face-to-face contact in the same airspace, but feeding, watering, sampling and environmental cleaning was carried out separately. The three experimentally infected goats did not show clinical signs of BTV, however high levels of viral RNA were detected and virus was isolated from their blood. At 21 dpi viral RNA was detected in, and virus was isolated from the blood of the three direct contact goats, which also seroconverted. The four indirect barrier contact goats remained uninfected throughout the duration of the experiment. In order to assess replication in a laboratory model species of Culicoides biting midge, more than 300 Culicoides sonorensis were fed a BTV-26 spiked blood meal and incubated for 7 days. The dissemination of BTV-26 in individual C. sonorensis was inferred from the quantity of virus RNA and indicated that none of the insects processed at day 7 possessed transmissible infections. This study shows that BTV-26 is easily transmitted through direct contact transmission between goats, and the strain does not seem to replicate in C. sonorensis midges using standard incubation conditions.

Published

2014

13. Vaccination of horses with a recombinant modified vaccinia Ankara virus (MVA) expressing African horse sickness (AHS) virus major capsid protein VP2 provides complete clinical protection against challenge

Author

Peter P. C. Mertens, Eva Calvo-Pinilla, Berta Alberca, Elisenda Viaplana, Javier Castillo-Olivares, Alicia Urniza, Marta Cabana, Simon Gubbins, Katarzyna Bachanek-Bankowska, and Lorraine Frost

Subjects

Serotype, Male, Modified vaccinia Ankara, viruses, African Horse Sickness Virus, Alpha interferon, Vaccinia virus, Antibodies, Viral, Virus, Article, Microbiology, Neutralization Tests, Immunology and Microbiology(all), Animals, Horses, Viremia, Vaccines, Synthetic, Protection, General Veterinary, General Immunology and Microbiology, biology, Viral Vaccine, Public Health, Environmental and Occupational Health, virus diseases, Viral Vaccines, VP2, biology.organism_classification, veterinary(all), Virology, Antibodies, Neutralizing, Vaccination, Infectious Diseases, Molecular Medicine, African horse sickness, Capsid Proteins, Female, Vaccine

Abstract

Highlights • A recombinant modified Vaccinia Ankara virus expressing VP2 of African horse sickness virus serotype 9 was generated. • Four horses were vaccinated on days 0 and 20. Three unvaccinated controls were used. • Vaccinated and control horses were challenged intravenously with 107.4TCID50 of AHSV-9 on day 34 of the study. • At challenge, vaccinates had virus neutralising antibodies but were negative for antibodies to AHSV-VP7. • All vaccinates were completely protected against clinical signs of African horse sickness., African horse sickness virus (AHSV) is an arthropod-borne pathogen that infects all species of equidae and causes high mortality in horses. Previously, a recombinant modified vaccinia Ankara (MVA) virus expressing the protein VP2 of AHSV serotype 4 was shown to induce virus neutralising antibodies in horses and protected interferon alpha receptor gene knock-out mice (IFNAR −/−) against virulent AHSV challenge. This study builds on the previous work, examining the protective efficacy of MVA-VP2 vaccination in the natural host of AHSV infection. A study group of 4 horses was vaccinated twice with a recombinant MVA virus expressing the major capsid protein (VP2) of AHSV serotype 9. Vaccinated animals and a control group of unvaccinated horses were then challenged with a virulent strain of AHSV-9. The vaccinated animals were completely protected against clinical disease and also against viraemia as measured by standard end-point dilution assays. In contrast, all control horses presented viraemia after challenge and succumbed to the infection. These results demonstrate the potential of recombinant MVA viruses expressing the outer capsid VP2 of AHSV as a protective vaccine against AHSV infection in the field.