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5. Field Application of qPCR Monitoring of Infectious Laryngotracheitis Virus in Settled Chicken House Dust and Its Role in Control of a Major Outbreak

Author

Awol M, Assen, Peter J, Groves, Ashley, Etherington, Priscilla F, Gerber, Margaret, Sexton, Sarah, Williamson, and Stephen W, Walkden-Brown

Subjects
Herpesvirus 1, Gallid, General Immunology and Microbiology, Food Animals, Drinking Water, Animals, Dust, Viral Vaccines, Animal Science and Zoology, Herpesviridae Infections, Vaccines, Attenuated, Chickens, Poultry Diseases, Disease Outbreaks
Abstract

Population-level sampling based on qPCR detection of infectious laryngotracheitis virus (ILTV) in poultry dust can be used to assess ILT vaccination outcomes following mass administration in drinking water. We report on the field application of this approach to assess the success of vaccine administration and its use in ILT outbreak control in meat chickens. In Study 1, dust samples were collected from 26 meat chicken flocks at 0, 4, 7, 14, and 21 days post drinking water vaccination (DPV) given between 7 to 13 days of age with the Serva or A20 live attenuated ILT vaccines. Unexpectedly, ILTV DNA was detected in dust samples collected prior to vaccination in 22/26 flocks. Typing revealed that the detected ILTV was different from the vaccine virus. To determine whether the detected ILTV DNA was from active infection or carryover of a noninfectious virus, Study 2 was implemented in 14 additional flocks with dust samples collected at 0, 7, 14, and 21 DPV and tracheal swabs collected from 15 birds/flock at 0 and 21 DPV. The results indicated that there was active infection with ILTV in those flocks before vaccination. This approach contributed to a statewide control program resulting in the eradication of ILT from South Australia as confirmed by negative ILTV test results for dust samples from 50 flocks and the absence of clinical ILT. These findings show that ILTV infection prior to vaccination is common in outbreak situations and that dust samples must be collected at 0 and 7 DPV for meaningful interpretation of vaccination outcomes and ILTV status. Comparatively low-cost dust testing during an outbreak, coupled with typing information, greatly assisted with decision making and control strategies during a major outbreak, including confirmation of the absence of infection in the final stages.Aplicación de campo del monitoreo por qPCR del virus de la laringotraqueítis infecciosa en el polvo de casetas avícolas y su función en el control de un brote importante El muestreo a nivel de población basado en la detección por qPCR del virus de la laringotraqueítis infecciosa (ILTV) en el polvo de instalaciones avícolas se puede utilizar para evaluar los resultados de la vacunación contra esta enfermedad después de la administración masiva en el agua de bebida. Se reporta la aplicación de campo de este enfoque para evaluar el éxito de la administración de vacunas y su uso en el control de brotes por laringotraqueítis infecciosa en pollos de engorde. En el Estudio 1, se recolectaron muestras de polvo de 26 parvadas de pollos de engorda a los 0, 4, 7, 14 y 21 días después de la vacunación en el agua de bebida (DPV) a los 7 a 13 días de edad con las vacunas de laringotraqueítis vivas atenuadas Serva o A20. Inesperadamente, se detectó ADN del virus de laringotraqueítis en muestras de polvo recolectadas antes de la vacunación en 22/26 parvadas. La tipificación reveló que el virus detectado era diferente del virus de la vacuna. Para determinar si el ADN del virus de laringotraqueítis detectado procedía de una infección activa o del remanente de un virus no infeccioso, se implementó el Estudio 2 en 14 parvadas adicionales con muestras de polvo recolectadas a los 0, 7, 14 y 21 días después de la vacunación y de hisopos traqueales recolectados de 15 aves/parvada a los cero y 21 días después de la vacunación. Los resultados indicaron que había infección activa con el virus de laringotraqueítis en esas parvadas antes de la vacunación. Este enfoque contribuyó a un programa de control estatal que resultó en la erradicación de laringotraqueítis del sur de Australia, como lo confirmaron los resultados negativos de las pruebas del mismo virus para muestras de polvo de 50 parvadas y la ausencia de laringotraqueítis infecciosa clínica. Estos hallazgos muestran que la infección por el virus de la laringotraqueítis antes de la vacunación es común en situaciones de brotes y que las muestras de polvo deben recolectarse a los cero y 7 días después de la vacunación para una interpretación significativa de los resultados de la vacunación y el estado de esta enfermedad. Las pruebas de polvo comparativamente de bajo costo durante un brote, junto con la información de tipificación, ayudaron mucho con la toma de decisiones y con las estrategias de control durante un brote importante, incluida la confirmación de la ausencia de infección en las etapas finales.

Published
2022
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11. Circulation and Molecular Characterization of Hemorrhagic Enteritis Virus in Commercial Turkey and Meat Chicken Flocks in Australia

Author

Priscilla F. Gerber, Stephen Spatz, Peter Gray, Sheridan Alfirevich, and Stephen W. Walkden-Brown

Subjects
Turkeys, Meat, General Immunology and Microbiology, Food Animals, Australia, Animals, Animal Science and Zoology, Chickens, Enteritis, Poultry Diseases, Siadenovirus
Abstract

Currently, there is no available vaccine against hemorrhagic enteritis virus (HEV) in Australia. Although it is assumed that subclinical HEV infections occur and may be associated with an increase in colibacillosis in Australian commercial turkey flocks, the prevalence of infection with this virus in the country is largely unknown. The aims of this study were to determine the extent of HEV infection in commercial flocks in Australia and to investigate the diversity of Australian HEV strains. Serum and spleen samples were collected from breeder and grower turkeys and serum was collected from breeder and grower chickens by the two major poultry integrator companies in Australia. Of the turkey samples, 727/849 (86%) sera were positive for anti-HEV antibodies by ELISA. HEV DNA was detected in 215/278 (77%) spleen samples positive by PCR. Of the meat chicken sera, 115/144 (80%) samples were seropositive. Sequencing the whole genome of three HEV field isolates showed that the Australian strains are highly similar and cluster separately from strains from other geographic regions although several point mutations were shared with HEV strains considered to be virulent. In conclusion, HEV infection is ubiquitous in Australian commercial poultry flocks. The impact of the many genomic point mutations detected in Australian HEV strains on virus pathogenicity is unclear.Circulación y caracterización molecular del virus de la enteritis hemorrágica en parvadas comerciales de pavo y pollos de engorde en Australia. Actualmente, no existe una vacuna disponible contra el virus de la enteritis hemorrágica (HEV) en Australia. Aunque se supone que se producen infecciones subclínicas por el virus de la enteritis hemorrágica y pueden estar asociadas con un aumento de la colibacilosis en las parvadas comerciales de pavos australianos, se desconoce en gran medida la prevalencia de la infección por este virus en el país. Los objetivos de este estudio fueron determinar la diseminación de la infección por el virus de la enteritis hemorrágica en parvadas comerciales en Australia e investigar la diversidad de cepas del virus de la enteritis hemorrágica australianas. Se recolectaron muestras de suero y bazo de pavos reproductores y de engorda y las dos principales empresas integradoras avícolas de Australia recolectaron suero de pollos reproductores y de engorde. De las muestras de pavo, 727/849 (86%) sueros fueron positivos para anticuerpos contra la enteritis hemorrágica por ELISA. Se detectó ADN del virus de la enteritis hemorrágica en 215/278 (77%) muestras de bazo positivas por PCR. De los sueros de carne de pollo, 115/144 (80%) muestras fueron seropositivas. La secuenciación del genoma completo de tres aislados de campo del virus de la enteritis hemorrágica mostró que las cepas australianas son muy similares y se agrupan por separado de las cepas de otras regiones geográficas, aunque se compartieron varias mutaciones puntuales con las cepas del virus de la enteritis hemorrágica consideradas virulentas. En conclusión, la infección por el virus de la enteritis hemorrágica es ubicua en las parvadas avícola comerciales australianas. No está claro el impacto de las diferentes mutaciones puntuales genómicas detectadas en las cepas australianas del virus de la enteritis hemorrágica sobre la patogenicidad del virus.

Published
2021

12. Detection and Quantification of Clostridium perfringens and Eimeria spp. in Poultry Dust Using Real-Time PCR Under Experimental and Field Conditions

Author

Sue M. Sharpe, C. Keerqin, Sarah L. Williamson, Natalie Morgan, Priscilla F. Gerber, Sosthene Musigwa, Alip Kumar, Sarbast K. Kheravii, Shu-Biao Wu, Stephen W. Walkden-Brown, and Ahaduzzaman

Subjects
Veterinary medicine, General Immunology and Microbiology, biology, 040301 veterinary sciences, Inoculation, animal diseases, 0402 animal and dairy science, Broiler, food and beverages, 04 agricultural and veterinary sciences, Clostridium perfringens, biology.organism_classification, medicine.disease, medicine.disease_cause, 040201 dairy & animal science, Eimeria, 0403 veterinary science, Coccidiosis, Real-time polymerase chain reaction, Food Animals, medicine, Animal Science and Zoology, Flock, Field conditions
Abstract

Infection of poultry with Eimeria spp., the causative agent of coccidiosis, can predispose birds to necrotic enteritis (NE) caused by netB gene-positive strains of Clostridium perfringens. The detection of Eimeria spp., C. perfringens, and netB were examined in settled dust from broiler flocks under experimental and field conditions. Dust samples were collected from settle plates twice weekly from two experimental flocks inoculated with three species of pathogenic Eimeria in 9-day-old chicks, followed by netB gene-positive C. perfringens 5 days later to produce subclinical and clinical NE. A noninoculated flock was sampled weekly from day 0 and served as a control flock. An additional 227 dust samples from commercial broiler flocks were collected at the end-of-batch (6-7 wk of age; one scraped dust sample per flock). In the NE-subclinical and NE-clinical flocks, high levels of Eimeria spp. and C. perfringens were detected after inoculation followed by a gradual decline over time. In the control flock, C. perfringens and netB were detected at low levels. No significant effect of sampling location was evident on Eimeria spp., C. perfringens, and netB load within poultry houses. These results provide evidence that Eimeria spp., C. perfringens, and netB gene copies can be readily measured in poultry dust samples collected in settle plates and may provide an alternative sampling method for monitoring flock coccidiosis and NE status. Further studies are required to assess the utility for such a test in commercial flocks.

Published
2020
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13. Airborne Transmission of Vaccinal and Wild Type Infectious Laryngotracheitis Virus and Noninfectivity of Extracts of Excreta from Infected Chickens

Author

Stephen W. Walkden-Brown, Shahid Nazir, Priscilla F. Gerber, and Addisu A. Yegoraw

Subjects
040301 veterinary sciences, Biology, Vaccines, Attenuated, Airborne transmission, 0403 veterinary science, Vaccine strain, Herpesvirus 1, Gallid, Food Animals, Animals, Infective virus, Poultry Diseases, Infectious laryngotracheitis virus, Differential transmission, General Immunology and Microbiology, Transmission (medicine), digestive, oral, and skin physiology, 0402 animal and dairy science, Wild type, Viral Vaccines, Herpesviridae Infections, 04 agricultural and veterinary sciences, 040201 dairy & animal science, Virology, Real-time polymerase chain reaction, Animal Science and Zoology, Chickens
Abstract

Infectious laryngotracheitis virus (ILTV) is thought to exit the host in respiratory aerosols and enter by inhalation of these. High levels of ILTV DNA have been detected in excreta, raising the possibility of alternative routes of shedding from the host. However, it is not known whether or not the ILTV DNA in excreta represents infective virus. This study investigated transmission of wild type and vaccinal ILTV from infected to susceptible commercial meat chickens. Airborne- and excreta-mediated transmission of two field isolates of ILTV (Classes 9 and 10) and three vaccine strains (SA2, A20, and Serva) were tested. To test airborne transmission, air from isolators containing infected birds was ducted through a paired isolator containing uninfected chickens. To test excreta transmission, aliquots were prepared from excreta containing a high level of ILTV DNA within the first week after infection. Chicks were infected bilaterally by eye drop. Clinical signs were monitored daily and choanal cleft swab samples for ILTV detection by quantitative PCR were collected at 4, 8, 15, 22, and 28 days postinfection (DPI) in the airborne transmission study and at 7 and 14 DPI from the excreta transmission studies. There was no transmission of ILTV from excreta, suggesting that ILTV is inactivated during passage through the gut. All strains of ILTV were transmitted by the airborne route but only to a limited extent for the vaccine viruses. The field viruses induced clinical signs, pathology, and greatly elevated ILTV genome copies in swabs. In summary, these findings confirm the suspected airborne transmission of ILTV, demonstrate differential transmission potential between wild type and vaccine strains by this route, and indicate that excreta is unlikely to be important in the transmission of ILTV and the epidemiology of ILT.

Published
2020
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14. Detection and Quantification of

Author

Md, Ahaduzzaman, Chake, Keerqin, Alip, Kumar, Sosthene, Musigwa, Natalie, Morgan, Sarbast K, Kheravii, Sue, Sharpe, Sarah, Williamson, Shu-Biao, Wu, Stephen W, Walkden-Brown, and Priscilla F, Gerber

Subjects
Enterotoxins, Clostridium perfringens, Coccidiosis, Bacterial Toxins, Clostridium Infections, Animals, Dust, Eimeria, New South Wales, Real-Time Polymerase Chain Reaction, Chickens, Poultry Diseases
Abstract

Infection of poultry with

Published
2020

15. Genomic Stability for PCR Detection of Infectious Laryngotracheitis Virus and Infectious Bronchitis Virus in Poultry Dust Samples Stored Under Different Conditions

Author

Awol M. Assen, Addisu A. Yegoraw, Priscilla F. Gerber, Stephen W. Walkden-Brown, and Thanh T. Tran

Subjects
Veterinary medicine, General Immunology and Microbiology, Moisture, Strain (chemistry), Inoculation, Bird Diseases, Infectious bronchitis virus, RNA virus, Dust, Genome, Viral, Herpesviridae Infections, Biology, biology.organism_classification, Polymerase Chain Reaction, Virus, Genomic Instability, Specimen Handling, Real-time polymerase chain reaction, Food Animals, Herpesvirus 1, Gallid, Animals, Animal Science and Zoology, Coronavirus Infections, Infectious laryngotracheitis virus
Abstract

Dust collected from the poultry house has been increasingly used as a population-level sample to monitor the presence of pathogens or to evaluate the administration of live vaccines. However, there are no guidelines for the storage of this sample type. This study investigated the stability of infectious laryngotracheitis virus (ILTV), a DNA virus, and infectious bronchitis virus (IBV), an RNA virus, in poultry dust kept under temperature and moisture conditions that mimic on-farm and laboratory storage. Dust samples were collected from chicks spray vaccinated with a live IBV vaccine and inoculated with a field ILTV strain via eye drop. Samples were stored under different moisture conditions (dry = 2% moisture, moist = 22%-71% moisture) and temperatures (-20, 4, 25, and 37 C) for different durations (0, 7, and 14 days, and 1, 2, 3, and 4 mo) in a factorial arrangement, followed by quantitative PCR for detection of virus genome copies (GC). The length of storage, moisture level, and storage temperature affected the viral genome load for ILTV and IBV but did not affect the number of positive samples for each virus. All treatment combinations were ILTV positive for at least 4 mo. In dry dust samples, all storage temperatures or durations had quantifiable ILTV or IBV GC. Moisture addition had a detrimental effect on viral genome load, causing an overall reduction of 0.3 log 10 for ILTV GC (7.29 and 6.97 log 10, P = 0.0001), and 1.3 log 10 for IBV GC (5.95 and 4.66 log 10, P = 0.0001), which are unlikely to have biologic significance. In conclusion, dry dust can be stored at any temperature up to 37 C for at least 4 mo without loss in qPCR detection of ILTV or IBV GC. Collection or storage of moist dust should be avoided, or air drying prior to storage is recommended if only moist dust is available.

Published
2020

16. Propagation of an Avirulent Turkey Hemorrhagic Enteritis Virus Isolate in Chickens

Author

Margaret E. Katz, Mary McMillan, Mohammad F. Hossain, Susan Burgess, Steve W Walkden-Brown, Katrin Renz, Priscilla F. Gerber, Paul Reynolds, and Phuong Hoang

Subjects
Male, 0301 basic medicine, Turkeys, 040301 veterinary sciences, Adenoviridae Infections, Spleen, Biology, Antibodies, Viral, Liver weight, Virus, 0403 veterinary science, 03 medical and health sciences, Food Animals, Turkey adenovirus 3, medicine, Animals, Turkey hemorrhagic enteritis, Poultry Diseases, Siadenovirus, Hemorrhagic enteritis virus, Virulence, General Immunology and Microbiology, Inoculation, 04 agricultural and veterinary sciences, Virology, Specific Pathogen-Free Organisms, 030104 developmental biology, medicine.anatomical_structure, Real-time polymerase chain reaction, Female, Animal Science and Zoology, Chickens
Abstract

SUMMARY A series of studies were undertaken to optimize the propagation of hemorrhagic enteritis virus (HEV) in specific-pathogen-free (SPF) chickens. A total of 562 SPF chickens were orally inoculated with an Australian avirulent HEV isolate of turkey origin at 9, 14, 21, or 28 days of age with 5, 6, 7, or 8 log 10 genomic copies (GC), while 102 chickens served as uninfected controls. No clinical signs were observed in infected chickens. There was an inoculum-dose–dependent increase in the relative spleen and liver weight (P < 0.01). Relative spleen weight 7 days post-HEV inoculation was up to 85% higher in chickens that were inoculated with 6 to 7 GC compared with controls, with no further increase at higher doses. Relative liver weight increased up to 14% in chickens inoculated with 6 GC, with no further increase. Birds inoculated with a 7 GC dose had a higher frequency of HEV DNA-positive birds (77% to 86%) than birds inoculated with lower doses (33% to 59%; P < 0.01). The most efficient dose for live...

Published
2018
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17. Detection and Quantification of Clostridium perfringens and Eimeria spp. in Poultry Dust Using Real-Time PCR Under Experimental and Field Conditions

Author

Ahaduzzaman, Md, primary, Keerqin, Chake, additional, Kumar, Alip, additional, Musigwa, Sosthene, additional, Morgan, Natalie, additional, Kheravii, Sarbast K., additional, Sharpe, Sue, additional, Williamson, Sarah, additional, Wu, Shu-Biao, additional, Walkden-Brown, Stephen W., additional, and Gerber, Priscilla F., additional

Published
2020
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19. Detection and Quantification of Clostridium perfringens and Eimeria spp. in Poultry Dust Using Real-Time PCR Under Experimental and Field Conditions.

Author

Ahaduzzaman, Md, Keerqin, Chake, Kumar, Alip, Musigwa, Sosthene, Morgan, Natalie, Kheravii, Sarbast K., Sharpe, Sue, Williamson, Sarah, Wu, Shu-Biao, Walkden-Brown, Stephen W., and Gerber, Priscilla F.

Subjects
EIMERIA, CLOSTRIDIUM perfringens, DUST, NECROTIC enteritis, POULTRY, POULTRY housing, COCCIDIOSIS
Abstract

Copyright of Avian Diseases is the property of American Association of Avian Pathologists, Inc. and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published
2021
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20. Airborne Transmission of Vaccinal and Wild Type Infectious Laryngotracheitis Virus and Noninfectivity of Extracts of Excreta from Infected Chickens.

Author

Yegoraw, Addisu Awukew, Nazir, Shahid, Gerber, Priscilla F., and Walkden-Brown, Stephen W.

Subjects
AIRBORNE infection, EYE drops, SYMPTOMS, VIRAL vaccines, CHICKEN diseases, VIRUSES, CHICKENS
Abstract

Copyright of Avian Diseases is the property of American Association of Avian Pathologists, Inc. and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published
2021
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22. Turkey Hemorrhagic Enteritis Virus Can Be Titrated but Not Propagated in Chicken Embryos

Author

Stephen W. Walkden-Brown, Mary McMillan, Priscilla F. Gerber, Mohammad F. Hossain, and Margaret E. Katz

Subjects
040301 veterinary sciences, viruses, 030231 tropical medicine, Chick Embryo, Biology, Virus, 0403 veterinary science, 03 medical and health sciences, 0302 clinical medicine, Food Animals, In vivo, Animals, Turkey hemorrhagic enteritis, Poultry Diseases, Siadenovirus, General Immunology and Microbiology, Inoculation, Embryonated, virus diseases, Embryo, 04 agricultural and veterinary sciences, Virology, Chorioallantoic membrane, Real-time polymerase chain reaction, embryonic structures, Animal Science and Zoology, Chickens
Abstract

This study aimed to investigate the feasibility of propagating and titrating hemorrhagic enteritis virus (HEV) in chicken embryos. A total of 308 embryonated eggs were used. At 10 days of embryonic age, eggs were inoculated via allantoic sac or chorioallantoic membrane routes with non-heat-treated (live) HEV or heat-treated (dead) HEV or served as negative controls. Allantoic fluid retrieved at 0, 1, 3, 5, and 7 days postinoculation (dpi) was tested for HEV by quantitative PCR. Inoculation with HEV did not cause visible growth impairment or lesions in the chicken embryos. Overall, there was no difference in postinoculation mortality rates among groups sham-inoculated (6/30, 20.0%) or inoculated with live (34/252, 13.4%) or dead (3/ 26, 6.9%) HEV (El virus de la enteritis hemorrágica de los pavos puede ser titulado pero no propagado en embriones de pollo. Este estudio tuvo como objetivo investigar la viabilidad de propagar y titular al virus de la enteritis hemorrágica de los pavos (con las siglas en inglés HEV) en embriones de pollo. Se utilizaron un total de 308 huevos embrionados. A los 10 días de edad embrionaria, los huevos se inocularon por vía saco alantoideo o por la membrana corioalantoidea con el virus de la enteritis hemorrágica sin tratamiento térmico (vivo) o con un virus de la enteritis hemorrágica con tratamiento térmico (muerto) y algunos sirvieron como controles negativos. El fluido alantoideo recuperado a los cero, uno, tres, cinco y siete días después de la inoculación se analizó para detectar el VHE mediante un método cuantitativo de PCR. La inoculación con el virus de la enteritis hemorrágica no causó daños visibles en el crecimiento ni lesiones en los embriones de pollo. En general, no hubo diferencias en las tasas de mortalidad después de la inoculación entre los grupos con inoculación simulada (6/30, 20.0%) o inoculados con el virus vivo de la enteritis hemorrágica (34/252, 13.4%) o con el virus muerto (3/26, 6.9%) (

Published
2018
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23. Viral kinetics, shedding profile, and transmission of serotype 1 Marek's disease vaccine Rispens/CVI988 in maternal antibody-free chickens

Author

Stephen W. Walkden-Brown, Katrin Renz, Tanzila Islam, and Sithara Ralapanawe

Subjects
Serotype, Veterinary medicine, animal structures, Time Factors, Dander, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, Real-Time Polymerase Chain Reaction, Vaccines, Attenuated, Virus Replication, Virus, Viral Proteins, Food Animals, Marek Disease, Animals, Lymphocytes, Marek Disease Vaccines, Viral shedding, Herpesvirus 2, Gallid, Poultry Diseases, General Immunology and Microbiology, biology, Antibody titer, Dust, Feathers, Virology, Specific Pathogen-Free Organisms, Virus Shedding, Kinetics, Feather, visual_art, visual_art.visual_art_medium, biology.protein, Animal Science and Zoology, Antibody, Viral load, Chickens, Spleen
Abstract

SUMMARY. Probably the most effective current vaccine against Marek’s disease is the live Rispens (CVI988) attenuated serotype 1 Marek’s disease virus (MDV). It is unknown whether the currently available Rispens vaccines transmit effectively between chickens. To investigate the kinetics and shedding of three commercially available strains of this virus and the extent of lateral transmission, we measured the shedding rate in dander and the viral load in peripheral blood lymphocytes (PBLs) and feather tips over time. Four identical climate-controlled rooms were stocked with a total of 70 specific-pathogen-free chickens for 56 days. In each of three rooms, 10 chickens were vaccinated with one of the commercial vaccines at day old and left in contact with 10 unvaccinated chickens. The fourth room contained 10 unvaccinated control chickens. As determined by MDV-specific quantitative real-time polymerase chain reaction of weekly room dust and individual PBLs and feather tip samples, the vaccine virus was shed from the vaccinated chickens in dander from day 7 postvaccination and transmitted effectively from vaccinated to incontact chickens with a lag period of 2–3 wk. Viral load in PBLs and feather tips peaked at days 7 and 14, respectively, and declined thereafter, whereas viral load in dust increased rapidly to day 21 and then increased gradually thereafter. Antibody titer at day 56 was correlated with earlier measures of MDV load in PBLs but not feather tips or dust. These results show that currently available Rispens CVI988 vaccine virus is shed in significant quantities from vaccinated chickens and transmits effectively between chickens.

Published
2013

24. Prevalence of Marek's disease virus in different chicken populations in Iraq and indicative virulence based on sequence variation in the ecoRI-q (meq) gene

Author

Katrin Renz, Salih J. Wajid, Margaret E. Katz, and Stephen W. Walkden-Brown

Subjects
Veterinary medicine, animal structures, Sequence analysis, animal diseases, Molecular Sequence Data, Prevalence, Virulence, Spleen, Biology, Real-Time Polymerase Chain Reaction, Virus, Food Animals, medicine, Marek Disease, Animals, Amino Acid Sequence, Herpesvirus 2, Gallid, Phylogeny, Poultry Diseases, Marek's disease, General Immunology and Microbiology, Broiler, Oncogene Proteins, Viral, Sequence Analysis, DNA, biology.organism_classification, medicine.anatomical_structure, Cross-Sectional Studies, Iraq, Animal Science and Zoology, Flock, Chickens, Sequence Alignment
Abstract

A cross-sectional survey was conducted in six provinces in southern Iraq to determine the point prevalence of Marek's disease virus (MDV) in different chicken populations followed by sequencing the meq gene for phylogenetic analysis and virulence-associated polymorphisms. A total of 109 samples from unvaccinated flocks were analyzed comprising 52 dust and 30 spleen samples from commercial broiler farms and 27 spleens from local layer chickens purchased in the town markets. The overall prevalence of MDV was 49.5% with no significant differences between provinces (P = 0.08) or sample types (P = 0.89). Prevalence ranged from 36.8% in Karbala and Nasiriyah to 65% in Amarah. The percentages of positive samples were 59.1%, 46.7%, and 48.1% in broiler dust, broiler spleen, and layer spleen, respectively. The overall mean (+/- SEM) Log10 MDV viral copy number per milligram of dust or spleen as determined by quantitative PCR was 1.78 +/- 0.19, with no significant differences between provinces (P = 0.10) or sample types (P = 0.38). In positive samples only, the overall mean was 3.43 +/- 0.18. Sequencing of the meq gene from samples that showed high levels of MDV target in qPCR testing was attempted. Nine samples were sequenced. These sequences were compared with meq sequences of MDVs of different pathotype. All the Iraqi MDVs had a short meq gene of 897 base pairs because of the deletion of 123 bp relative to the reference strain Md5. The Iraqi meq sequences also contained single-nucleotide polymorphisms, resulting in differences in the amino acid sequence. All of the nine Iraqi meq genes encoded two repeats of four-proline sequences. The published negative association between four-proline repeat number and MDV virulence suggests that the Iraqi MDVs are likely to be highly virulent, but this needs to be confirmed by in vivo testing. Taken together, these results indicate that MDV is common in unvaccinated commercial and village chickens in southern Iraq, that there is limited meq gene sequence variation, that all sequenced samples had a short meq with two four-proline repeats, and that this is consistent with a high level of virulence.

Published
2013

25. Development, application, and results of routine monitoring of Marek's disease virus in broiler house dust using real-time quantitative PCR

Author

Stephen W. Walkden-Brown, Susan Burgess, Aminul Islam, Peter J. Groves, Sue M. Sharpe, and Ambrosio Rubite

Subjects
Serotype, Veterinary medicine, animal structures, Victoria, viruses, animal diseases, Biology, Real-Time Polymerase Chain Reaction, Sensitivity and Specificity, Virus, Herpesvirus 1, Meleagrid, Viral genetics, Food Animals, hemic and lymphatic diseases, Marek Disease, Animals, Herpesvirus 3, Gallid, Animal Husbandry, Herpesvirus 2, Gallid, Poultry Diseases, Marek's disease, General Immunology and Microbiology, Broiler, virus diseases, Reproducibility of Results, Dust, Oncogene Proteins, Viral, biology.organism_classification, Virology, Real-time polymerase chain reaction, Animal Science and Zoology, Seasons, Chickens, Spleen
Abstract

Results are presented from four studies between 2002 and 2011 into the feasibility of routinely monitoring Marek's disease virus serotype 1 (MDV-1) in broiler house dust using real-time quantitative PCR (qPCR) measurement. Study 1 on two farms showed that detection of MDV-1 occurred earlier on average in dust samples tested using qPCR than standard PCR and in spleen samples from five birds per shed assayed for MDV-1 by qPCR or standard PCR. DNA quality following extraction from dust had no effect on detection of MDV-1. Study 2 demonstrated that herpesvirus of turkeys (HVT) and MDV serotype 2 (MDV-2) in addition to MDV-1 could be readily amplified from commercial farm dust samples, often in mixtures. MDV-2 was detected in 11 of 20 samples despite the absence of vaccination with this serotype. Study 3 investigated the reproducibility and sensitivity of the qPCR test and the presence of inhibitors in the samples. Samples extracted and amplified in triplicate showed a high level of reproducibility except at very low levels of virus near the limit of detection. Mixing of samples prior to extraction provided results consistent with the proportions in the mixture. Tests for inhibition showed that if the template contained DNA in the range 0.5-20 ng/microl no inhibition of the reaction was detectable. The sensitivity of the tests in terms of viral copy number (VCN) per milligram of dust was calculated to be in the range 24-600 VCN/mg for MDV-1, 48-1200 VCN/mg for MDV-2, and 182-4560 VCN/mg for HVT. In study 4 the results of 1976 commercial tests carried out for one company were analyzed. Overall 23.1% of samples were positive for MDV-1, 26.1% in unvaccinated and 16.4% in vaccinated chickens. There was marked regional and temporal variation in the proportion of positive samples and the MDV-1 load. The tests were useful in formulating Marek's disease vaccination strategies. The number of samples submitted has increased recently, as has the incidence of positive samples. These studies provide strong evidence that detection and quantitation of MDV-1, HVT, and MDV-2 in poultry house dust using qPCR is robust, sensitive, reproducible, and meaningful, both biologically and commercially. Tactical vaccination based on monitoring of MDV-1 rather than routine vaccination may reduce selection pressure for increased virulence in MDV-1.

Published
2013

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