Your search keyword '"Reoviridae Infections diagnosis"' showing total 235 results

1. A σC-protein-based indirect enzyme-linked immunosorbent assay for clinical detection of antiavian reovirus antibodies.

Author

Yang X, Gao H, Cheng Z, Zhang S, Zhao Y, Zheng H, Gao L, Cao H, Li X, Zheng SJ, and Wang Y

Subjects

Animals, Sensitivity and Specificity, Orthoreovirus, Avian immunology, Enzyme-Linked Immunosorbent Assay veterinary, Enzyme-Linked Immunosorbent Assay methods, Chickens, Reoviridae Infections veterinary, Reoviridae Infections diagnosis, Reoviridae Infections immunology, Reoviridae Infections virology, Poultry Diseases diagnosis, Poultry Diseases virology, Poultry Diseases immunology, Antibodies, Viral blood

Abstract

Avian reovirus (ARV) is the causative agent of avian viral arthritis and causes significant economic losses to the global poultry industry. For clinical diagnosis, detecting ARV-specific antibodies is crucial. We successfully expressed the ARV-σC protein in insect cells using the baculovirus expression vector system, achieving an expression level of approximately 200 mg/L. We developed an indirect enzyme-linked immunosorbent assay (iELISA) using the ARV-σC protein as a coating antigen to detect antibodies against it. The inter-batch and intrabatch coefficients of iELISA variation were less than 10%. Its sensitivity (1:12,800 diluted in serum) was 4 times higher than that of the indirect immunofluorescence assay (IFA; 1:3200 diluted in serum), and it showed no cross-reactivity with antibodies against other common avian viruses (such as Infectious bursal disease virus, Newcastle disease virus). The practicality of the iELISA was further evaluated using clinical samples. 300 clinical sera from chickens vaccinated with the ARV attenuated vaccine and 20 SPF sera were tested using both the iELISA and the IFA, demonstrating a 100% conformity rate. In conclusion, these results suggest that the iELISA developed in this study is a rapid, sensitive, and specific method that could serve as an effective diagnostic tool for monitoring and controlling avian viral arthritis., Competing Interests: DISCLOSURES All authors disclosed no relevant relationships., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

2. Detection of avian reovirus (ARV) by ELISA based on recombinant σB, σC and σNS full-length proteins and protein fragments.

Author

de Matos TRA, Palka APG, de Souza C, Fragoso SP, and Pavoni DP

Subjects

Animals, Antibodies, Viral blood, Capsid Proteins immunology, Capsid Proteins genetics, Viral Proteins immunology, Viral Proteins genetics, Orthoreovirus, Avian immunology, Orthoreovirus, Avian genetics, Orthoreovirus, Avian isolation & purification, Enzyme-Linked Immunosorbent Assay methods, Enzyme-Linked Immunosorbent Assay veterinary, Chickens, Reoviridae Infections veterinary, Reoviridae Infections diagnosis, Poultry Diseases virology, Poultry Diseases diagnosis, Recombinant Proteins immunology

Abstract

Introduction. Avian reovirus (ARV) is associated with arthritis/tenosynovitis and malabsorption syndrome in chickens. The σC and σB proteins, both exposed to the virus capsid, are highly immunogenic and could form the basis for diagnostic devices designed to assess the immunological status of the flock. Gap Statement. Commercial ARV ELISAs cannot distinguish between vaccinated and infected animals and might not detect circulating ARV strains. Aim. We aimed to develop a customized test to detect the circulating field ARV strains as well as distinguish between vaccinated and unvaccinated animals. Methodology. We developed ELISA assays based on recombinant (r) σB, σC and the nonstructural protein σNS and tested them using antisera of vaccinated and unvaccinated chickens as well as negative controls. Fragments of σB and σC proteins were also used to study regions that could be further exploited in diagnostic tests. Results. Vaccinated and unvaccinated birds were positive by commercial ELISA, with no difference in optical density values. In contrast, samples of unvaccinated animals showed lower absorbance in the rσB and rσC ELISA tests and higher absorbance in the rσNS ELISA test than the vaccinated animals. Negative control samples were negative in all tests. Fragmentation of σB and σC proteins showed that some regions can differentiate between vaccinated and unvaccinated animals. For example, σB amino acids 128-179 (σB-F4) and σC amino acids 121-165 (σC-F4) exhibited 85 and 95% positivity among samples of vaccinated animals but only 5% and zero positivity among samples of unvaccinated animals, respectively. Conclusion. These data suggest that unvaccinated birds might have been exposed to field strains of ARV. The reduction in absorbance in the recombinant tests possibly reflects an increased specificity of our test since unvaccinated samples showed less cross-reactivity with the vaccine proteins immobilized on ELISAs. The discrepant results obtained with the protein fragment tests between vaccinated and unvaccinated animals are discussed in light of the diversity between ARV strains.

Published

2024

3. Real-Time RT-PCR Assays for Typing of Epizootic Hemorrhagic Disease Virus.

Author

Sailleau C, Zientara S, and Bréard E

Subjects

Animals, Reoviridae Infections veterinary, Reoviridae Infections virology, Reoviridae Infections diagnosis, RNA, Viral genetics, Hemorrhagic Disease Virus, Epizootic genetics, Hemorrhagic Disease Virus, Epizootic isolation & purification, Hemorrhagic Disease Virus, Epizootic classification, Real-Time Polymerase Chain Reaction methods, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

Real-time RT-PCR for the detection of epizootic hemorrhagic disease virus (EHDV) in clinical samples is a fast and sensitive tool for the diagnosis and confirmation of disease. Several real-time RT-PCR methods have been reported over the last 10 years. In this chapter, we describe seven duplex real-time RT-PCR assays to amplify part of genome segment 2 of EHDV to enable serotype identification. The assay includes the detection of an endogenous control gene-beta-actin., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

4. Virus Neutralization Test for Detecting and Quantifying Serum-Neutralizing Antibodies to Epizootic Hemorrhagic Disease Virus (EHDV) (Serotypes 1, 2, and 4-8).

Author

Savini G, Bonfini B, and Spedicato M

Subjects

Animals, Serogroup, Reoviridae Infections immunology, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Reoviridae Infections virology, Neutralization Tests methods, Antibodies, Neutralizing immunology, Antibodies, Neutralizing blood, Antibodies, Viral immunology, Antibodies, Viral blood, Hemorrhagic Disease Virus, Epizootic immunology

Abstract

The virus neutralization test (VNT) is a functional immunoassay which detects the presence and quantity of neutralizing antibodies. It is a highly sensitive and specific test. As with most neutralization assays, the EHDV VNT does not react with all virus-targeting antibodies, but specifically with those antibodies that bind to VP2, the outermost capsid structural protein of the virus. The interaction between VP2 and neutralizing antibodies can block EHDV cell binding, neutralizing its infectivity. The detection and quantification of neutralizing antibodies are indicative of how protected an animal is against reinfection. The EHD VNT can therefore be a useful tool to monitor the efficacy of a vaccination campaign. VP2 is also the main determinant of EHDV serotype specificity, and so EHDV-neutralizing antibodies which target VP2 are also serotype-specific. Throughdetecting and quantifying neutralizing antibodies, the VNT can discriminate the EHDV serotype responsible for an infection and provides insights into the time of infection. It is considered the gold standard test for identifying and quantifying antibodies against EHDV serotypes present in test serum samples. The assay is performed in vitro and is based on inhibition of virus infectivity in the presence of neutralizing antibodies. A neutralizing antibody titer is determined through the presence or absence of cytopathic effect in a cell monolayer. The VNT is a relatively inexpensive assay using standard laboratory equipment; however, to perform the assay, cell cultures, significant time, intensive labor, and technical skill are required., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

5. Rapid Laboratory Diagnosis of Epizootic Hemorrhagic Disease Virus Using a Loop-Mediated Isothermal Amplification Assay.

Author

Rajko-Nenow P and Flannery J

Subjects

Animals, Sensitivity and Specificity, DNA Primers genetics, RNA, Viral genetics, Nucleic Acid Amplification Techniques methods, Hemorrhagic Disease Virus, Epizootic genetics, Hemorrhagic Disease Virus, Epizootic isolation & purification, Molecular Diagnostic Techniques methods, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Reoviridae Infections virology

Abstract

Reverse transcriptase loop-mediated isothermal amplification (RT-LAMP) is a molecular diagnostic assay that is particularly useful for the detection of viral diseases of livestock. A major advantage of RT-LAMP is that it can be used either as a rapid field test or as a high-throughput screening tool in veterinary laboratories, with sensitivity comparable to the real-time RT-PCR assay. Unlike conventional or qPCR, RT-LAMP uses a strand displacement polymerase and a set of four to six primers that bind to several regions of the target nucleic acid. Amplification occurs without thermal cycling, and coupled with the numerous primers, RT-LAMP offers a rapid and highly specific molecular assay. In this chapter, we describe the RT-LAMP protocol for the detection of epizootic hemorrhagic disease virus (EHDV) as a low-cost, specific, and sensitive screening tool in veterinary diagnostic laboratories. We also provide guidance on how to adapt the RT-LAMP assay for rapid field testing., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

6. Detection of EHDV Antibodies Using Enzyme-Linked Immunosorbent Assay (ELISA).

Author

Batten C, Newbrook K, Loundras EA, and Frost L

Subjects

Animals, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Reoviridae Infections immunology, Reoviridae Infections virology, Sheep, Enzyme-Linked Immunosorbent Assay methods, Antibodies, Viral blood, Antibodies, Viral immunology, Hemorrhagic Disease Virus, Epizootic immunology

Abstract

Enzyme-linked immunosorbent assay (ELISA) is a relatively inexpensive, rapid, and high-throughput diagnostic tool to detect antibodies raised against epizootic hemorrhagic disease virus (EHDV) in ruminant serum. While the presence of EHDV antibodies only confirms prior exposure to the virus, it does not conclusively determine infection status. The c-ELISA can be used in conjunction with other diagnostic tests (e.g., real-time PCR) to reinforce diagnosis of infection or as a surveillance tool to support disease control. The EHDV competition ELISA (c-ELISA) described here is a commercial diagnostic assay, recommended by the World Organisation for Animal Health (WOAH), that detects ruminant antibodies against the highly conserved EHDV structural protein, VP7., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

7. Real-Time RT-PCR for the Diagnosis of Epizootic Hemorrhagic Disease Virus.

Author

Ashby M

Subjects

Animals, RNA, Viral genetics, Hemorrhagic Disease Virus, Epizootic genetics, Hemorrhagic Disease Virus, Epizootic isolation & purification, Real-Time Polymerase Chain Reaction methods, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Reoviridae Infections virology, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

Real-time reverse transcription-polymerase chain reaction (real-time RT-PCR) has become an essential tool in rapid and reliable detection of animal diseases such as epizootic hemorrhagic disease (EHD). Here we provide a protocol for the detection of epizootic hemorrhagic disease virus (EHDV) genetic material in blood and tissue samples, using a real-time RT-PCR that targets a conserved region in segment 9 of the EHDV genome. This protocol can be used to detect up to approximately 90 samples in a single run and can be completed in less than 4 h., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

8. End-Point RT-PCR Assays for Detection and Typing of Epizootic Hemorrhagic Disease Virus.

Author

Sailleau C, Zientara S, and Bréard E

Subjects

Animals, Reoviridae Infections veterinary, Reoviridae Infections virology, Reoviridae Infections diagnosis, RNA, Viral genetics, Genome, Viral, Serotyping methods, Hemorrhagic Disease Virus, Epizootic genetics, Hemorrhagic Disease Virus, Epizootic isolation & purification, Hemorrhagic Disease Virus, Epizootic classification, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

The emergence of EHDV in Europe during the autumn of 2022 reinforces the need for molecular tools (RT-PCR) for rapid detection of animals infected with this virus. Viral genome testing can be performed on whole blood under anticoagulant, spleen, and bloody organ homogenates from ruminants. It can also be performed on cell culture following viral isolation tests. Various so-called classical or end-point RT-PCRs will be described, which permit the amplification of a part of the viral genome (targeting segment 7) allowing the detection of EHDV whatever the serotype (pan-RT-PCR) and also to amplify a portion of the gene coding the viral protein (VP) 2 enabling serotyping. The PCR amplification products are visualized by agarose gel electrophoresis. Sequencing of the type-specific RT-PCR amplification products allows for the serotype of the virus to be determined., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

9. [Emergence of epizootic hemorrhagic disease in Europe].

Author

Zientara S, Bréard E, Vitour D, and Sailleau C

Subjects

Animals, Cattle, Ruminants, Europe epidemiology, Sicily, Deer, Reoviridae Infections epidemiology, Reoviridae Infections veterinary, Reoviridae Infections diagnosis, Hemorrhagic Disorders

Abstract

Epizootic hemorrhagic disease (EHD) is a non-contagious arthropod-borne disease transmitted by blood-sucking midges of the genus Culicoides. It affects domestic and wild ruminants, mainly white-tailed deer and cattle. At the end of October and in November 2022, outbreaks of EHD were confirmed in several cattle farms in Sardinia and Sicily. This is the first detection of EHD in Europe. The loss of free status and the lack of effective prophylactic measures could have significant economic consequences for infected countries.

Published

2023

10. Development of a rapid and sensitive reverse transcription real-time quantitative PCR assay for detection and quantification of grass carp reovirus II.

Author

Li J, Wu H, Xu W, Wang Y, Wang H, Wang Y, Li Y, Shi C, Bergmann SM, Mo X, Wang Q, and Yin J

Subjects

Animals, Reverse Transcription, Real-Time Polymerase Chain Reaction, Antibodies, Viral, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Carps, Reoviridae genetics, Fish Diseases diagnosis

Abstract

Hemorrhagic disease of grass carp, which is induced by grass carp reovirus II (GCRV-II), leads to mass mortality in grass carp culture and causes enormous economic loss. However, there is currently no quantitative analysis method for the detection of GCRV-II, which is greatly restricted the etiological and epidemiological study of the disease. In this study a reverse transcription TaqMan PCR (RT-qPCR) assay was developed for the quantitative detection of GCRV-II. The probe and primers targeted location is the segment 6 (S6) region of the GCRV-II genome which is highly conserved. Standard curves were drawn and criteria were confirmed after the determination of the optimum reaction conditions. The species-specific assay showed that the method is highly specific and has no cross reactions with other pathogens. The assay was sufficiently sensitive to detect as low as 10 copies of virus RNA. Moreover, the method has a very good repeatability for batches and inter-batches sample detection. Then the method was applied to detect the virus in tissue samples from clinically infected grass carp, compared with conventional RT-seminested PCR, the RT-qPCR represents a specific value for detection rate of positive samples. In summary, the RT-qPCR was applied and achieved high sensitivity and specificity for GCRV-II detection., (Copyright © 2022 Elsevier B.V. All rights reserved.)

Published

2023

11. Emergence of epizootic hemorrhagic disease in Europe.

Author

Zientara S, Bréard E, Vitour D, and Sailleau C

Subjects

Animals, Cattle, Ruminants, Europe epidemiology, Sicily, Deer, Reoviridae Infections epidemiology, Reoviridae Infections veterinary, Reoviridae Infections diagnosis, Hemorrhagic Disorders

Abstract

Epizootic hemorrhagic disease (EHD) is a non-contagious arthropod-borne disease transmitted by blood-sucking midges of the genus Culicoides. It affects domestic and wild ruminants, mainly white-tailed deer and cattle. At the end of October and in November 2022, outbreaks of EHD were confirmed in several cattle farms in Sardinia and Sicily. This is the first detection of EHD in Europe. The loss of free status and the lack of effective prophylactic measures could have significant economic consequences for infected countries.

Published

2023

12. Development of a wide-range real-time RT-PCR assay for detection of Avian reovirus (ARV).

Author

Farnoushi Y, Heller D, and Lublin A

Subjects

Animals, Reverse Transcriptase Polymerase Chain Reaction, Reproducibility of Results, Chickens, Sensitivity and Specificity, RNA, Orthoreovirus, Avian genetics, Poultry Diseases diagnosis, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Nucleic Acids

Abstract

Avian reovirus (ARV) is a common pathogen in chickens and other birds causing a variety of clinical symptoms such as arthritis and tenosynovitis but also enteric and respiratory symptoms. A rapid method that detects as many ARV genotypes as possible, will contribute to the early identification and control of the virus infection that causes high economic damage to the poultry industry worldwide. In this study, a real-time reverse transcription polymerase chain reaction (RT-qPCR) assay for the detection of ARV was developed. The RT-qPCR detection threshold for ARV genomic RNA standard cases was 10 copies/µL. Reproducibility of the RT-qPCR was confirmed by intra- and inter-assays. When the nucleic acids of different ARV genotypes and other common avian pathogens (IBDV, AIV, NDV, and IBV) were subjected to that RT-qPCR test, only ARV samples tested positive while all other pathogens tested negative. Due to the simplicity, convenience, high sensitivity, and specificity of the assay, the probe-based RT-qPCR is proposed to be used as an alternative diagnostic assay for the detection of ARVs in veterinary diagnostic laboratories., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2022 Elsevier B.V. All rights reserved.)

Published

2022

13. Avian Reoviruses from Clinical Cases of Tenosynovitis: An Overview of Diagnostic Approaches and 10-Year Review of Isolations and Genetic Characterization.

Author

Sellers HS

Subjects

Male, Female, Animals, Chickens, Lameness, Animal, Poultry, Turkeys, Antibodies, Viral, Tenosynovitis veterinary, Orthoreovirus, Avian genetics, Autovaccines, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Poultry Diseases diagnosis, Poultry Diseases epidemiology, Poultry Diseases prevention & control, Arthritis, Infectious veterinary

Abstract

Reoviral-induced tenosynovitis/viral arthritis is an economically significant disease of poultry. Affected birds present with lameness, unilateral or bilateral swollen hock joints or shanks, and/or reluctance to move. In severe cases, rupture of the gastrocnemius or digital flexor tendons may occur, and significant culling may be necessary. Historically, vaccination with a combination of modified live and inactivated vaccines has successfully controlled disease. Proper vaccination reduced vertical transmission and provided maternal-derived antibodies to progeny to protect against disease, at an age when they were most susceptible. Starting in 2011-2012, an increased incidence of tenosynovitis/viral arthritis was observed in chickens and turkeys. In chickens, progeny from reovirus-vaccinated breeders were affected, suggesting commercial vaccines did not provide adequate protection against disease. In turkeys, clinical disease was primarily in males, although females can also be affected. The most significant signs were observed around 14-16 wks of age and include reluctance to move, lameness, and limping on one or both legs. The incidence of tenosynovitis/viral arthritis presently remains high. Reoviruses isolated from clinical cases are genetically and antigenically characterized as variants, meaning they are different from vaccine strains. Characterization of the field isolates reveals multiple new genotypes and serotypes that are significantly different from commercial vaccines and each other. In 2012, a single prevalent virus was isolated from a majority of the cases submitted to the Poultry Diagnostic and Research Center at the University of Georgia. Genetic characterization of the σC protein revealed the early isolates belonged to genetic cluster (GC) 5. Soon after the initial identification of the GC5 variant reovirus, many broiler companies incorporated these isolates from their farms into their autogenous vaccines and continue to do so today. The incidence of GC5 field isolates has decreased significantly, likely because of the widespread use of the isolates in autogenous vaccines. Unfortunately, variant reoviruses belonging to multiple GCs have emerged, despite inclusion of these isolates in autogenous vaccines. In this review, an overview of nomenclature, sample collection, and diagnostic testing will be covered, and a summary of variant reoviruses isolated from clinical cases of tenosynovitis/viral arthritis over the past 10 yrs will be provided.

Published

2022

14. Development of an indirect enzyme-linked immunosorbent assay for the detection of novel chicken orthoreovirus.

Author

Liu H, Wei Z, Yang J, Wang Y, Hu J, Tang Y, and Diao Y

Subjects

Animals, Antibodies, Viral, Chickens, Enzyme-Linked Immunosorbent Assay methods, Enzyme-Linked Immunosorbent Assay veterinary, Sensitivity and Specificity, Viral Proteins, Orthoreovirus, Orthoreovirus, Avian, Poultry Diseases diagnosis, Reoviridae Infections diagnosis, Reoviridae Infections veterinary

Abstract

A novel avian orthoreovirus (N-ARV) variant characterized with obvious arthritis and synovial inflammation, was isolated from Shandong, China in May 2016. It caused chicken poor growth and enormous economic losses to the poultry industry of China. However, there are few effective methods for detecting the antibody levels of N-ARV. In this study, a viral structural protein σC was expressed using the prokaryotic expression vector pET32a (+). The target protein was obtained by inducing for 6 hours at an IPTG concentration of 0.6mM. The optimal dilution of the coating antigen and serum antibody were determined to be 1000 fold and 10 fold respectively. A specificity test showed that there was no positive reactivity between N-ARV and other pathogens, and when the positive serum was diluted 100 times detection results were still checkable. The repeatability of this method was determined by the inter assay and intra assay tests with variability ranging from 4.85% to 7.93%. In conclusion, this indirect enzyme linked immunosorbent assay (ELISA) will be useful for large-scale serological surveys and monitoring antibody levels in N-ARV infection., (Copyright© by the Polish Academy of Sciences.)

Published

2022

15. Development of a Novel Loop Mediated Isothermal Amplification Assay (LAMP) for the Rapid Detection of Epizootic Haemorrhagic Disease Virus.

Author

Rajko-Nenow P, Howson ELA, Clark D, Hilton N, Ambagala A, Svitek N, Flannery J, and Batten C

Subjects

Animals, Bluetongue virology, Cattle, DNA Primers genetics, Deer, RNA, Viral genetics, Real-Time Polymerase Chain Reaction, Reverse Transcription, Sensitivity and Specificity, Hemorrhagic Disease Virus, Epizootic isolation & purification, Molecular Diagnostic Techniques methods, Nucleic Acid Amplification Techniques methods, Reoviridae Infections diagnosis, Reoviridae Infections virology

Abstract

Epizootic haemorragic disease (EHD) is an important disease of white-tailed deer and can cause a bluetongue-like illness in cattle. A definitive diagnosis of EHD relies on molecular assays such as real-time RT-qPCR or conventional PCR. Reverse transcription loop-mediated isothermal amplification (RT-LAMP) is a cost-effective, specific, and sensitive technique that provides an alternative to RT-qPCR. We designed two sets of specific primers targeting segment-9 of the EHD virus genome to enable the detection of western and eastern topotypes, and evaluated their performance in singleplex and multiplex formats using cell culture isolates (n = 43), field specimens (n = 20), and a proficiency panel (n = 10). The limit of detection of the eastern and western RT-LAMP assays was estimated as ~24.36 C T and as ~29.37 C T in relation to real-time RT-qPCR, respectively, indicating a greater sensitivity of the western topotype singleplex RT-LAMP. The sensitivity of the western topotype RT-LAMP assay, relative to the RT-qPCR assay, was 72.2%, indicating that it could be theoretically used to detect viraemic cervines and bovines. For the first time, an RT-LAMP assay was developed for the rapid detection of the EHD virus that could be used as either a field test or high throughput screening tool in established laboratories to control the spread of EHD.

Published

2021

16. Isolation of epizootic hemorrhagic disease virus serotype 7 from cattle showing fever in Japan in 2016 and improvement of a reverse transcription-polymerase chain reaction assay to detect epizootic hemorrhagic disease virus.

Author

Yamamoto K, Hiromatsu R, Kaida M, Kato T, Yanase T, and Shirafuji H

Subjects

Animals, Cattle, Japan epidemiology, Reverse Transcriptase Polymerase Chain Reaction veterinary, Reverse Transcription, Serogroup, Cattle Diseases diagnosis, Cattle Diseases epidemiology, Hemorrhagic Disease Virus, Epizootic genetics, Reoviridae Infections diagnosis, Reoviridae Infections epidemiology, Reoviridae Infections veterinary

Abstract

Epizootic hemorrhagic disease (EHD) is an arthropod-borne disease of wild and domestic ruminants caused by the EHD virus (EHDV). To date, seven EHDV serotypes have been identified. In Japan, strain Ibaraki of EHDV serotype 2 has caused outbreaks of Ibaraki disease in cattle. In addition, EHDV serotype 7 (EHDV-7) has caused large-scale EHD epizootics. In mid-September 2016, eight cattle at a breeding farm in Fukuoka Prefecture, Japan developed fever. Since EHDV-7 was detected in sentinel cattle in western Japan in 2016, we suspected that the cause of this fever might be an EHDV-7 infection. In this study, we tested cattle for EHDV-7 and some other viruses. Consequently, EHDV was isolated from washed blood cells collected from three of the eight cattle, and genetic analysis of genome segment 2 revealed that this isolate was EHDV-7. Moreover, all affected cattle tested positive for anti-EHDV-7 neutralizing antibodies. Our results suggest that the fever was caused by EHDV-7 infection. In addition, we modified a conventional reverse transcription polymerase chain reaction assay for the specific detection of EHDV. This modified assay could detect various strains of EHDV isolated in Japan, Australia, and North America. Furthermore, the assay permitted the detection of EHDV-7 in blood cells collected from seven of the eight cattle. We believe that this modified assay will be a useful tool for the diagnosis of EHD.

Published

2021

17. Development and evaluation of recombinase polymerase amplification combined with lateral flow dipstick assays for co-detection of epizootic haemorrhagic disease virus and the Palyam serogroup virus.

Author

Li ZR, Yang ZX, Li ZH, Gao X, Hu ZY, Yang H, and Liao DF

Subjects

Animals, Biological Assay veterinary, Cattle, Hemorrhagic Disease Virus, Epizootic genetics, Nucleic Acid Amplification Techniques methods, Palyam Virus genetics, Real-Time Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction veterinary, Recombinases, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Sensitivity and Specificity, Serogroup, Serologic Tests methods, Hemorrhagic Disease Virus, Epizootic isolation & purification, Nucleic Acid Amplification Techniques veterinary, Palyam Virus isolation & purification, Serologic Tests veterinary

Abstract

Background: Epizootic haemorrhagic disease virus (EHDV) and the Palyam serogroup viruses (PALV) have led to significant economic losses associated with livestock production globally. A rapid, sensitive and specific method for the detection of EHDV and PALV is critical for virus detection, monitoring, and successful control and elimination of related diseases., Results: In the present study, a recombinase polymerase amplification combined with lateral flow dipstick (RPA-LFD) assay for the co-detection of genome segment 1 (Seg-1) of EHDV and PALV was developed and evaluated. The analytical sensitivities of the established RPA-LFD assay in the detection of EHDV and PALV were 7.1 copies/µL and 6.8 copies/µL, respectively. No cross-reaction with other members of the genus Orbivirus, including African horse sickness virus, bluetongue virus, Guangxi orbivirus, Tibet orbivirus and Yunnan orbivirus was observed. The established RPA-LFD assay accurately detected 39 EHDV strains belonging to 5 serotypes and 29 PALV strains belonging to 3 serotypes. The trace back results of quantitative real-time polymerase chain reaction (qRT-PCR) and the established RPA-LFD assay on sentinel cattle were consistent. The coincidence rates of qRT-PCR and the established RPA-LFD assay in 56 blood samples from which EHDV or PALV had been isolated and 96 blood samples collected from cattle farms were more than 94.8 %. The results demonstrated that the established RPR-LFD assay is specific, sensitive and reliable, and could be applied in early clinical diagnosis of EHDV and PALV., Conclusions: This study highlights the development and application of the RPA-LFD assay in the co-detection of EHDV and PALV for the first time. The assay could be used as a potential optional rapid, reliable, sensitive and low-cost method for field diagnosis of EHDV and PALV., (© 2021. The Author(s).)

Published

2021

18. New insights on Avian orthoreovirus and Chicken astrovirus co-infection in an Italian broiler flock: preliminary biomolecular and pathological results.

Author

Stamilla A, Messina A, Puleio R, Loria GR, Antoci F, Giuseppe C, and Lanza M

Subjects

Animals, Astroviridae Infections complications, Astroviridae Infections diagnosis, Avastrovirus genetics, Coinfection, Diagnosis, Differential, Orthoreovirus, Avian genetics, Polymerase Chain Reaction veterinary, Poultry Diseases virology, RNA, Viral analysis, Reoviridae Infections complications, Reoviridae Infections diagnosis, Sicily, Astroviridae Infections veterinary, Avastrovirus isolation & purification, Chickens, Orthoreovirus, Avian isolation & purification, Poultry Diseases diagnosis, Reoviridae Infections veterinary

Abstract

Common pathogens of intensive poultry farms, either parasitic or bacterial, such as Coccidiaor Salmonella, are well known and strictly controlled by veterinary management. This case study reports an unusual case of runting stunting syndrome (RSS) observed on a Sicilian poultry farm of broiler chickens during 2019. The investigation was carried out on five chickens which present delayed in body weight and growth performance. Animals showed also difficulty in deambulation and diarrhea. At necropsy, intestinal lesions were detected in three of the five clinical cases. Gut samples were collected and analyzed to identify potential pathogens responsible for the RSS. Presence of viruses was detected by using quantitative reverse transcription PCR (RT‑qPCR), while selected tissues were fixed and embedded in paraffin wax according to routine procedures. All histological sections were stained with hematoxylin‑eosin. RT‑qPCR successfully detected both Chicken astrovirus (CAstV) and Avian orthoreovirus (ARV). Histology evidenced severe specific lesions on the intestinal mucosa in liver and kidneys. Chicken astrovirus and Avian orthoreovirus RNA was also detected in cecal tonsils, kidney and liver, thus implying their possible primary role in inducing the disease. Further studies are needed to evaluate the role of other possible factors (low biosecurity measures, e.g.) and, most of all, the consequences in terms of economic losses and animal health impairment.

Published

2021

19. Generation and characterization of aptamers against grass carp reovirus infection for the development of rapid detection assay.

Author

Yu Q, Liu M, Wu S, Xiao H, Qin X, and Li P

Subjects

Animals, Cells, Cultured, Fish Diseases virology, Molecular Probes, Nucleic Acid Conformation, Reoviridae Infections diagnosis, SELEX Aptamer Technique, Aptamers, Nucleotide, Carps virology, Fish Diseases diagnosis, Reoviridae Infections veterinary

Abstract

Grass carp reovirus (GCRV) causes devastating viral haemorrhagic disease in farmed grass carp (Ctenopharyngon idellus). As novel molecular probes, aptamers have been widely applied in rapid diagnosis and efficient therapies against virus or diseases. In this study, three single-stranded DNA (ssDNA) aptamers were selected against GCRV-infected CIK cells via SELEX (systematic evolution of ligands by exponential enrichment technology). Secondary structures predicted by MFOLD indicated that aptamers formed stem-loop structures, and GVI-11 had the lowest ΔG value of -30.84 KJ/mol. Three aptamers could specifically recognize GCRV-infected CIK cells, with calculated dissociation constants (Kd) of 220.86, 176.63 and 278.66 nM for aptamers GVI-1, GVI-7 and GVI-11, respectively, which indicated that they could serve as specific delivery system for antiviral therapies. The targets of aptamers GVI-1, GVI-7 and GVI-11 on the surface of GCRV-infected cells could be membrane proteins, which were trypsin-sensitive. Furthermore, FAM-labelled aptamer GVI-7 could be applied to detect GCRV infection in vivo. It is the first time to generate and characterize aptamers against GCRV-infected cells. These aptamers have great potentials in development of rapid diagnosis technology and antiviral agents against GCRV infection in aquaculture., (© 2020 John Wiley & Sons Ltd.)

Published

2021

20. Evaluation of a commercial ELISA for detection of epizootic haemorrhagic disease antibodies in domestic and wild ruminant sera.

Author

Bréard E, Viarouge C, Donnet F, Sailleau C, Rossi S, Pourquier P, Vitour D, Comtet L, and Zientara S

Subjects

Animals, Bluetongue diagnosis, Cattle, Deer, Goats, Reagent Kits, Diagnostic veterinary, Reoviridae Infections diagnosis, Reoviridae Infections virology, Serologic Tests veterinary, Sheep, Antibodies, Viral blood, Bluetongue virology, Capsid Proteins immunology, Enzyme-Linked Immunosorbent Assay veterinary, Hemorrhagic Disease Virus, Epizootic immunology, Reoviridae Infections veterinary, Ruminants virology

Abstract

Bluetongue (BT) and epizootic haemorrhagic disease (EHD) are vector-borne viral diseases affecting domestic and wild ruminants. Both are notifiable under OIE rules. BT and EHD viruses (BTV and EHDV) are closely related Orbiviruses with structural, antigenic and molecular similarities. Both viruses can produce analogous clinical signs in susceptible animals. Serological tests are commonly used for BT and EHD diagnosis and surveillance. Competitive ELISA (c-ELISA) is the most widely used serological test for the specific detection of BTV or EHDV viral protein 7 (VP7) antibodies (Abs). The specificity and sensitivity of the BTV c-ELISA kits available on the market are recognized for the detection of BTV Abs. Concerning EHD, a single commercial EHDV c-ELISA kit (ELISA A kit) commonly used for diagnosis in Europe and Africa was available between 2011 and 2018 but is now no longer on the market. In this study, we evaluated a new commercial c-ELISA to detect ruminant EHDV VP7 Abs in 2,199 serum samples from cattle, sheep, goats, wild deer and zoo animals. The results showed that this ELISA kit is specific and can detect the presence of IgG anti-EHDV VP7 with a very good diagnostic specificity and a satisfactory sensitivity in domestic ruminants, zoo animals and wild deer. Therefore, the evaluated c-ELISA can detect the introduction of EHDV into an area where BTV-seropositive domestic animals are present. The performance of this kit is similar to that of the c-ELISA A kit and can thus be used for diagnosis., (© 2020 Blackwell Verlag GmbH.)

Published

2020

21. A TaqMan-based real-time PCR assay for specific detection of novel duck reovirus in China.

Author

Zhang S, Li W, Liu X, Li X, Gao B, Diao Y, and Tang Y

Subjects

Animals, China, Ducks, Poultry Diseases diagnosis, Real-Time Polymerase Chain Reaction methods, Reoviridae Infections diagnosis, Reoviridae Infections virology, Reproducibility of Results, Sensitivity and Specificity, Orthoreovirus, Avian isolation & purification, Poultry Diseases virology, Real-Time Polymerase Chain Reaction veterinary, Reoviridae Infections veterinary

Abstract

Background: In China, Newly emerging duck reovirus (NDRV) variants have been causing major disease problems in cherry valley ducks. NDRV has the potential to cause high morbidity and 5-50% mortality rates. Severe hemorrhagic-necrosis in the liver and spleen were commonly seen in NDRV affected ducks. The availability of upgraded methods for rapid diagnosis of newly emerging DRV variants is crucial for successful DRV infection control and prevention., Results: In this study, we present a TaqMan-based real-time PCR assay (RT-qPCR) for the detection of NDRV infection. Using the conserved regions within the NDRV genome, we designed the specific primers and probe. The lower limit of detection for NDRV infection was 10 copies/μL (Ct values: 38.3) after the optimization of the RT-qPCR conditions. By cross-checking with other duck viral pathogens, no cross-reactivity was observed confirming the assay was highly specific for the detection of NDRV. Reproducibility of the RT-qPCR was confirmed by intra- and inter-assay variability was less than 2.91%(Intra-assay variability of Ct values: 0.07-1.48%; Interassay variability of Ct values: 0.49-2.91%). This RT-qPCR and conventional PCR (cPCR) detected one hundred and twenty samples of NDRV infection from different regions. The result shows that the positive rates were 94.17 and 84.17% respectively. The detection rate of RT-qPCR rapid detection assay was 10% higher than that of the cPCR method., Conclusion: This research developed a highly sensitive, specific, reproducible and versatile of RT-qPCR for quantitatively detecting NDRV. It can be used to study the pathogenesis and epidemiology investigation of NDRV.

Published

2020

22. A real-time reverse-transcription isothermal recombinase polymerase amplification assay for the rapid detection of genotype III grass carp (Ctenopharyngodon idella) reovirus.

Author

Wang H, Zhou S, Wen J, Sun M, Jiang Y, Lu L, and Xie J

Subjects

Animals, Antibodies, Viral, Cell Line, Fish Diseases diagnosis, Fish Diseases virology, Genotype, Molecular Diagnostic Techniques methods, Reoviridae classification, Reoviridae isolation & purification, Reoviridae Infections diagnosis, Reoviridae Infections virology, Reverse Transcription, Sensitivity and Specificity, Carps virology, DNA-Directed DNA Polymerase genetics, Recombinases genetics, Reoviridae genetics, Reoviridae Infections veterinary

Abstract

Grass carp (Ctenopharyngodon idella) hemorrhagic disease, which is characterized by external and internal hemorrhage, is a serious infectious disease affecting grass carp production. Strains of the causative agent, grass carp reovirus (GCRV), are divided into genotypes I, II and III, which are represented by the isolates GCRV-873, GCRV-HZ08 and GCRV-104, respectively. In this study, a real-time reverse-transcription recombinase polymerase amplification (real-time RT-RPA) assay was developed to detect the genotype III grass carp reovirus GCRV-104. The assay was based on the detection of the vp55 gene which encodes the outer fiber protein of the virus. A portable ESE-Quant Tube scanner, with a dimension of 17.4 × 18.8 cm, weighing about 1 kg, and equipped with temperature settings to amplify the DNA isothermally and spectral devices to detect the amplified products using fluorescence, was used to complete the assay. Under the optimal conditions, the assay took approximately 10 min to complete at 37 °C and showed no cross-reactions with other aquatic viruses. Consequently, this rapid real-time RT-RPA assay is a useful method for the simple, rapid and reliable detection of genotype III GCRV strains in resource-limited diagnostic laboratories., Competing Interests: Declaration of Competing Interest We declare that we have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2020

23. Retrospective Analysis of Turkey Arthritis Reovirus Diagnostic Submissions in Minnesota.

Author

Barrera M, Kumar P, Porter RE, Goyal SM, and Mor SK

Subjects

Animals, Minnesota, Reoviridae Infections diagnosis, Retrospective Studies, Tenosynovitis diagnosis, Poultry Diseases diagnosis, Reoviridae isolation & purification, Reoviridae Infections veterinary, Tenosynovitis veterinary, Turkeys

Abstract

Turkey arthritis reovirus (TARV) causes tenosynovitis in turkeys, resulting in decreased profits for producers due to the increase in morbidity, mortality, and feed conversion ratio. There is limited information on TARV epidemiology, including the dynamics of diagnostic submissions to veterinary diagnostic laboratories. In this study, we retrospectively analyzed 719 cases of lameness in turkeys submitted to the Minnesota Veterinary Diagnostic Laboratory from March 2010 to May 2018. Almost all submissions were tendon pools, which were tested by virus isolation and/or real-time reverse transcription-polymerase chain reaction. Most of the submissions were from Minnesota. We found 52% of the submitted cases to be positive for TARV. The TARV-positive submissions increased considerably in the last few years. There was no statistical evidence that TARV diagnostic submissions were seasonal, although positive submissions were higher in January, April, July, and December. TARV-positive submissions also increased as flocks aged. In summary, we found that TARV submissions have increased in the last few years, have varied over time, and are correlated with age of the bird. This information is important guidance for conducting more studies to understand TARV infection dynamics.

Published

2019

24. Bluetongue virus and epizootic hemorrhagic disease virus survey in cattle of the Galapagos Islands.

Author

Vinueza RL, Cruz M, Bréard E, Viarouge C, and Zanella G

Subjects

Animals, Antibodies, Viral blood, Bluetongue diagnosis, Bluetongue virology, Cattle, Cattle Diseases diagnosis, Cattle Diseases virology, Ecuador epidemiology, Enzyme-Linked Immunosorbent Assay veterinary, Prevalence, Reoviridae Infections diagnosis, Reoviridae Infections epidemiology, Reoviridae Infections virology, Bluetongue epidemiology, Bluetongue virus isolation & purification, Cattle Diseases epidemiology, Hemorrhagic Disease Virus, Epizootic isolation & purification, Reoviridae Infections veterinary

Abstract

Bluetongue virus (BTV) and epizootic hemorrhagic disease virus (EHDV) have both been reported in mainland Ecuador, but their occurrence was unknown in the Galapagos Islands, an Ecuadorian province. We aimed to detect BTV or EHDV in cattle from the 3 main cattle-producing Galapagos Islands at a between-herd design prevalence of 20% and a within-herd design prevalence of 15%. Blood samples were collected from 410 cattle in 33 farms and tested for antibodies against BTV and EHDV by competitive ELISAs. All results were negative, suggesting that BTV and EHDV are not present in the Galapagos Islands.

Published

2019

25. Development of a VP38 recombinant protein-based indirect ELISA for detection of antibodies against grass carp reovirus genotype II (iELISA for detection of antibodies against GCRV II).

Author

Zeng W, Wang Y, Guo Y, Bergmann SM, Yin J, Li Y, Ren Y, Shi C, and Wang Q

Subjects

Animals, Blotting, Western methods, Enzyme-Linked Immunosorbent Assay methods, Fish Diseases virology, Fluorescent Antibody Technique, Indirect methods, Recombinant Proteins metabolism, Reoviridae Infections diagnosis, Reoviridae Infections virology, Sensitivity and Specificity, Viral Proteins metabolism, Antibodies, Viral isolation & purification, Blotting, Western veterinary, Enzyme-Linked Immunosorbent Assay veterinary, Fish Diseases diagnosis, Fluorescent Antibody Technique, Indirect veterinary, Reoviridae isolation & purification, Reoviridae Infections veterinary

Abstract

Currently, serological assays for grass carp reovirus genotype II (GCRV-II) diagnosis are not available. In this study, an indirect enzyme-linked immunosorbent assay (ELISA) for the detection of antibodies against GCRV-II was developed. The structural protein VP38 of GCRV-II was used as the coating antigen. Monoclonal antibodies (mAb) against IgM of grass carp labelled with HRP were used as a secondary antibody. The antigen concentration and serum dilution were optimized using chess board titration. Furthermore, the specificity of indirect ELISA assay was confirmed by cross check with sera positive for other grass carp pathogens. In comparison with results obtained from indirect immunofluorescence assay (IFA) and Western blot by testing of 60 serum samples to evaluate the sensitivity and specificity of the ELISA, agreement between 90% and 96.7% was reached, respectively. A serological survey was performed using the assay with grass carp field serum samples. The seropositive rate of the 242 serum samples was 69.8%. In conclusion, the developed indirect ELISA is a very specific and sensitive test that will be useful for large-scale serological surveys to detect indirectly GCRV II infections as well as to monitor the changes of antibody level after immunization., (© 2018 John Wiley & Sons Ltd.)

Published

2018

26. Development of an indirect ELISA assay for detecting antibodies against mammalian reovirus in pigs.

Author

Li Z, Zhang X, Hu X, Tian J, Kang H, Guo D, Liu J, and Qu L

Subjects

Animals, Fluorescent Antibody Technique, Indirect, Neutralization Tests, Reoviridae isolation & purification, Reoviridae Infections diagnosis, Reoviridae Infections immunology, Serogroup, Swine virology, Swine Diseases virology, Viral Fusion Proteins immunology, Antibodies, Viral blood, Enzyme-Linked Immunosorbent Assay methods, Reoviridae immunology, Reoviridae Infections veterinary, Swine Diseases diagnosis

Abstract

Mammalian reovirus (MRV) infects many species. Over the past decades, MRV infections in pigs have been reported, and several highly pathogenic MRV strains have recently been isolated in the United States. In this study, an indirect enzyme-linked immunosorbent assay (ELISA) against the σ1 protein from a serotype 3 reovirus strain (MPC/04) was established to detect antibodies in pigs. The assay did not react with antisera against other pig pathogens and was consistent with the indirect immunofluorescence assay (IFA) and virus neutralization test (VNT). In conclusion, the assay is specific and highly sensitive, providing a method for large-scale monitoring of the serotype 3 MRV infection epidemiology in pigs., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

27. A multiplex xTAG assay for the simultaneous detection of five chicken immunosuppressive viruses.

Author

Cong F, Zhu Y, Wang J, Lian Y, Liu X, Xiao L, Huang R, Zhang Y, Chen M, and Guo P

Subjects

Animals, Birnaviridae Infections diagnosis, Birnaviridae Infections virology, Chickens virology, Circoviridae Infections diagnosis, Circoviridae Infections virology, Coinfection diagnosis, Coinfection virology, Marek Disease virology, Microarray Analysis methods, Multiplex Polymerase Chain Reaction methods, Poultry Diseases virology, Reoviridae Infections diagnosis, Reoviridae Infections virology, Reproducibility of Results, Retroviridae Infections diagnosis, Retroviridae Infections virology, Sensitivity and Specificity, Tumor Virus Infections diagnosis, Tumor Virus Infections virology, Birnaviridae Infections veterinary, Chicken anemia virus, Circoviridae Infections veterinary, Coinfection veterinary, Infectious bursal disease virus, Mardivirus, Marek Disease diagnosis, Microarray Analysis veterinary, Multiplex Polymerase Chain Reaction veterinary, Orthoreovirus, Avian, Poultry Diseases diagnosis, Reoviridae Infections veterinary, Reticuloendotheliosis Viruses, Avian, Retroviridae Infections veterinary, Tumor Virus Infections veterinary

Abstract

Background: Chicken anemia virus (CAV), avian reovirus (ARV), infectious bursal disease virus (IBDV), Marek's disease virus (MDV) and reticuloendotheliosis virus (REV) all cause immunosuppressive disease in birds through vertical or horizontal transmission. Mixed infections with these immunosuppressive pathogens lead to atypical clinical signs and obstruct accurate diagnoses and epidemiological investigations. Therefore, it is essential to develop a high-throughput assay for the simultaneous detection of these immunosuppressive viruses with high specificity and sensitivity. The aim of this study was to establish a novel method using a RT-PCR assay combined with fluorescence labeled polystyrene bead microarray (multiplex xTAG assay) to detect single or mixed viral infections., Results: The results showed that the established xTAG assay had no nonspecific reactions with avian influenza virus (AIV), infectious bronchitis virus (IBV), newcastle disease virus (NDV), infectious laryngotracheitis virus (ILTV), Mycoplasma gallisepticum (MG) and Mycoplasma synoviae (MS). The limit of detection was 1.0 × 10 3 copies/μL for IBDV and 1.0 × 10 2 copies/μL for the other four viruses. Ninety field samples were tested and the results were confirmed using conventional RT-PCR methods. The detection results of these two methods were 100% consistent. The established multiplex xTAG assay allows a high throughput and simultaneous detection of five chicken immunosuppressive viruses., Conclusion: The multiplex xTAG assay has been showed to be an additional tool for molecular epidemiology studies of five chicken immunosuppressive viruses in the poultry industry.

Published

2018

28. Detection of mammalian orthoreovirus type-3 (Reo-3) infections in mice based on serotype-specific hemagglutination protein sigma-1.

Author

Fingas F, Volke D, Bielefeldt P, Hassert R, and Hoffmann R

Subjects

Animals, Chromatography, High Pressure Liquid, Enzyme-Linked Immunosorbent Assay, Hemagglutination, Hemagglutination Tests, Mice, Reoviridae Infections diagnosis, Serogroup, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Tandem Mass Spectrometry, Viral Core Proteins genetics, Mammalian orthoreovirus 3 classification, Reoviridae Infections immunology, Reoviridae Infections virology, Viral Core Proteins immunology

Abstract

Background: Reovirus type-3 infections cause severe pathologies in young mice and thus influence animal experiments in many ways. Therefore, the Federation of Laboratory Animal Science Associations (FELASA) recommends an annual screening in laboratory mice as part of a thorough health monitoring program. Based on the high protein sequence homology among the different reovirus serotypes, immunofluorescence antibody assay and other indirect methods relying on the whole virus are presumably cross-reactive to antibodies triggered by mammalian orthoreovirus infections independent of the serotype., Methods: The serotype-specific protein σ-1 was expressed in Escherichia coli with an N-terminal Strep-tag and a C-terminal His-tag. The purified Strep-rσ-1-His-construct was used to develop an indirect ELISA by testing defined positive and negative sera obtained by experimental infection of mice as well as field sera., Results: The Strep-rσ-1-His-ELISA provided high sensitivity and specificity during validation. Notably, a high selectivity was also observed for sera positively tested for other relevant FELASA-listed pathogens. Screening of field samples indicated that a commercial reovirus type-3-based ELISA might be cross-reactive to other murine reovirus serotypes and thus produces false-positive results., Conclusions: The prevalence of reovirus type-3 might be overestimated in German animal facilities and most likely in other countries as well. The occurrence of other reovirus serotypes, however, raises the question if murine health monitoring programs should be extended to these pathogens.

Published

2018

29. Development of a recombinant σB protein based dot-ELISA for the diagnosis of avian reovirus (ARV).

Author

Majumder S, Chauhan TKS, Nandi S, Goswami PP, Tiwari AK, Dhama K, Mishra BP, and Kumar D

Subjects

Animals, Chickens, Orthoreovirus, Avian immunology, Poultry Diseases virology, Reoviridae Infections diagnosis, Sensitivity and Specificity, Antibodies, Viral blood, Antigens, Viral immunology, Enzyme-Linked Immunosorbent Assay methods, Orthoreovirus, Avian isolation & purification, Poultry Diseases diagnosis, Reoviridae Infections veterinary

Abstract

Avian reovirus (ARV) causes significant economic losses to the poultry industry worldwide. The ARV proteins fall into three different classes based on their sizes:λ (large); μ (medium) and σ (small). σB, an outer capsid protein of the ARV contains group specific neutralizing epitopes and induces strong immune response in naturally infected chickens. This study describes the development of a rapid dot-enzyme linked immunosorbent assay (dot-ELISA) using recombinant σB protein antigen of 54 kDa (approx). The assay is rapid (4-5 h) and results can be read by the naked eye. Sixteen ARV positive serum samples (group A) produced strong reaction in the dot-ELISA while twenty of the ARV negative serum samples (group B) collected from SPF chickens showed no reaction. Seventy six randomly collected serum samples were tested with a commercial indirect ELISA kit and the in-house developed dot-ELISA. A total of sixty eight serum samples were found to be positive by indirect ELISA and sixty five serum samples were found to be positive by dot-ELISA. Therefore, using the commercial ELISA as the reference test, the dot-ELISA had a diagnostic sensitivity of 83.8% and specificity of 88.6%. This dot-ELISA can be used as a simple, reliable and inexpensive alternative to commercial ELISA kits for serodiagnosis of ARV where the facilities for standard ELISA are not available., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

30. Development of indirect immunofluorescence assay for TCID 50 measurement of grass carp reovirus genotype II without cytopathic effect onto cells.

Author

Wang Q, Xie H, Zeng W, Wang L, Liu C, Wu J, Wang Y, Li Y, and Bergmann SM

Subjects

Animals, Antibodies, Viral, Cell Culture Techniques, Cell Line, China, Cytopathogenic Effect, Viral, Fish Diseases diagnosis, Fish Diseases virology, Genes, Viral genetics, Real-Time Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction veterinary, Reoviridae Infections veterinary, Reoviridae Infections virology, Sensitivity and Specificity, Carps virology, Fluorescent Antibody Technique, Indirect methods, Fluorescent Antibody Technique, Indirect veterinary, Genotype, Reoviridae genetics, Reoviridae isolation & purification, Reoviridae Infections diagnosis

Abstract

Grass carp reovirus (GCRV) caused severe hemorrhagic disease with significant losses of fingerling and yearling grass carp, Cyenopharyngodon idellus, in southeast Asian. It was first isolated in 1983 in China, and clade analysis of the different GCRV isolates indicates there are at least three different genotypes I, II, and III. In recent years, GCRV genotype II has been determined as a dominant virus type which cause severe obvious clinical signs in fish but no cytopathic effect onto presently available cell culture. TCID 50 is one of standard method to quantity infectious virus particles. In the present study, an indirect immunofluorescence assay (IFA) was developed using antibody against a protein encoded by segment 10 of GCRV genotype II. Moreover, the specific assay to differentitate GCRV of different genotypes and a sensitive assay for determination of GCRV genotype II were developed respectively. The results showed the IFA only can recognize genotype II virus at the lowest initial concentration of 550 genomic copies/ml. Furthermore, comparison of results obtained from qPCR and the TCID 50 assay combined IFA was conducted. The results indicated that TCID 50 of GCRV isolates JX0901 and HZ08 differs with 2 log steps reduction in the numbers of viruses compared with the number of genome copies detected by qPCR. The immunofluorescence assay developed is sensitive, specific, and the TCID 50 combined with IFA will be a standardizable technique for the quantitation and detection of infectious GCRV in cell culture without cytolysis., (Copyright © 2017. Published by Elsevier Ltd.)

Published

2018

31. VIRUS ISOLATION AND MOLECULAR DETECTION OF BLUETONGUE AND EPIZOOTIC HEMORRHAGIC DISEASE VIRUSES FROM NATURALLY INFECTED WHITE-TAILED DEER (ODOCOILEUS VIRGINIANUS).

Author

Kienzle C, Poulson RL, Ruder MG, and Stallknecht DE

Subjects

Animals, Bluetongue diagnosis, Bluetongue virus genetics, Cattle, Freezing, Hemorrhagic Disease Virus, Epizootic genetics, Lung virology, RNA, Viral isolation & purification, Reagent Kits, Diagnostic, Real-Time Polymerase Chain Reaction veterinary, Reoviridae Infections diagnosis, Reoviridae Infections virology, Retrospective Studies, Reverse Transcriptase Polymerase Chain Reaction veterinary, Spleen virology, Bluetongue virology, Bluetongue virus isolation & purification, Deer, Hemorrhagic Disease Virus, Epizootic isolation & purification, Reoviridae Infections veterinary

Abstract

Hemorrhagic disease in North America is caused by multiple serotypes of epizootic hemorrhagic disease virus (EHDV) and bluetongue virus (BTV). Diagnostic tests for detection of EHDV and BTV include virus isolation (VI), reverse transcriptase (RT)-PCR, and real-time RT-PCR (rRT-PCR). Our objective was to compare the diagnostic capabilities of three rRT-PCR protocols for detection of EHDV and BTV from naturally infected white-tailed deer (Odocoileus virginianus). We compared the effectiveness of these assays to traditional viral detection methods (e.g., VI) for historic and current clinical cases. Because of the variable nature of tissue collection and storage before diagnostic testing, an evaluation of viral persistence on multiple freeze-thaw events was also conducted. Two of the rRT-PCR assays provided for reliable detection of EHDV and BTV from 100% of clinically affected and VI-confirmed infected animals. Additionally, no significant change in viral titer was observed on multiple freeze-thaw events.

Published

2017

32. Competitive enzyme-linked immunosorbent assay using baculovirus-expressed VP7 for detection of epizootic haemorrhagic disease virus (EHDV) antibodies.

Author

Forzan M, Pizzurro F, Zaccaria G, Mazzei M, Spedicato M, Carmine I, Salini R, Tolari F, Cerri D, Savini G, and Lorusso A

Subjects

Animals, Animals, Domestic immunology, Animals, Domestic virology, Animals, Wild immunology, Animals, Wild virology, Antigens, Viral immunology, Recombinant Proteins immunology, Reoviridae Infections diagnosis, Reoviridae Infections immunology, Reoviridae Infections virology, Ruminants immunology, Ruminants virology, Sf9 Cells, Viral Core Proteins genetics, Antibodies, Viral blood, Baculoviridae genetics, Enzyme-Linked Immunosorbent Assay methods, Hemorrhagic Disease Virus, Epizootic immunology, Reoviridae Infections veterinary, Viral Core Proteins immunology

Abstract

Epizootic haemorrhagic disease (EHD) is a vector-borne infectious viral disease of domestic and wild ruminants. EHD could spread from infected northern African countries in free territories like the EU; therefore, the availability of diagnostic assays would represent key components for adequate surveillance and control programs. In this study, the gene encoding the VP7 protein of EHD virus (EHDV) was expressed into a baculovirus-infected insect cell system. With this unpurified protein we developed a home-made competitive ELISA (cELISA) and a total number of 275 serum samples, originating from domestic and wild ruminants, were tested. 74/275 were previously shown to be positive for EHDV antibodies by a commercially available ELISA kit. A "very good" agreement was demonstrated when compared to a commercial ELISA kit (Cohen's kappa value=0.832). Samples which caused disagreement between the two assays originated from wildlife which highlights the need for further validation by using serum samples from wild animals., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

33. A convenient immunochromatographic test strip for rapid detection of Scylla serrata reovirus.

Author

Fan D, Liu J, Xu M, Yuan Y, Yang J, and Chen J

Subjects

Animals, Antibodies, Viral immunology, Mice, Rabbits, Sensitivity and Specificity, Brachyura virology, Chromatography, Affinity, Reagent Kits, Diagnostic veterinary, Reoviridae immunology, Reoviridae Infections diagnosis

Published

2017

34. Development of Real-Time RT-PCR Assays for Detection and Typing of Epizootic Haemorrhagic Disease Virus.

Author

Maan NS, Maan S, Potgieter AC, Wright IM, Belaganahalli M, and Mertens PPC

Subjects

Animals, Polymerase Chain Reaction veterinary, Reoviridae Infections diagnosis, Reoviridae Infections veterinary, Ceratopogonidae virology, Hemorrhagic Disease Virus, Epizootic isolation & purification, Veterinary Medicine methods, Viral Proteins genetics

Abstract

Epizootic haemorrhagic disease virus (EHDV) is an emerging arboviral pathogen of wild and domestic ruminants worldwide. It is closely related to bluetongue virus (BTV) and is transmitted by adult females of competent Culicoides vector species. The EHDV genome consists of ten linear double-stranded (ds)RNA segments, encoding five non-structural and seven structural proteins. Genome-segment reassortment contributes to a high level of genetic variation in individual virus strains, particularly in the areas where multiple and distinct virus lineages co-circulate. In spite of the relatively close relationship between BTV and EHDV herd-immunity to BTV does not appear to protect against the introduction and infection of animals by EHDV. Although EHDV can cause up to 80% morbidity in affected animals, vaccination with the homologous EHDV serotype is protective. Outer-capsid protein VP2, encoded by Seg-2, is the most variable of the EHDV proteins and determines both the specificity of reactions with neutralizing antibodies and consequently the identity of the eight EHDV serotypes. In contrast, VP6 (the viral helicase), encoded by Seg-9, is highly conserved, representing a virus species/serogroup-specific antigen. We report the development and evaluation of quantitative (q)RT-PCR assays targeting EHDV Seg-9 that can detect all EHDV strains (regardless of geographic origin/topotype/serotype), as well as type-specific assays targeting Seg-2 of the eight EHDV serotypes. The assays were evaluated using orbivirus isolates from the 'Orbivirus reference collection' (ORC) at The Pirbright Institute and were shown to be EHDV pan-reactive or type-specific. They can be used for rapid, sensitive and reliable detection and identification (typing) of EHDV RNA from infected blood, tissue samples, homogenized Culicoides, or tissue culture supernatant. None of the assays detected RNA from closely related but heterologous orbiviruses, or from uninfected host animals or cell cultures. The techniques presented could be used for both surveillance and vaccine matching (serotype identification) as part of control strategies for incursions in wild and domestic animal species., (© 2016 The Authors. Transboundary and Emerging Diseases Published by Blackwell Verlag GmbH.)

Published

2017

35. Infection experiments with novel Piscine orthoreovirus from rainbow trout (Oncorhynchus mykiss) in salmonids.

Author

Hauge H, Vendramin N, Taksdal T, Olsen AB, Wessel Ø, Mikkelsen SS, Alencar ALF, Olesen NJ, and Dahle MK

Subjects

Animals, Denmark, Fish Diseases diagnosis, Fish Diseases transmission, Fish Proteins blood, Fish Proteins genetics, Gene Expression, Heart virology, Hemoglobins analysis, Host-Pathogen Interactions, Muscle, Skeletal virology, Norway, Oncorhynchus mykiss blood, Oncorhynchus mykiss genetics, Orthoreovirus genetics, Orthoreovirus pathogenicity, RNA, Viral genetics, Reoviridae Infections diagnosis, Reoviridae Infections transmission, Reverse Transcriptase Polymerase Chain Reaction, Salmo salar blood, Salmo salar genetics, Virulence, Fish Diseases virology, Oncorhynchus mykiss virology, Orthoreovirus physiology, Reoviridae Infections virology, Salmo salar virology

Abstract

A new disease in farmed rainbow trout (Onchorhyncus mykiss) was described in Norway in 2013. The disease mainly affected the heart and resembled heart and skeletal muscle inflammation (HSMI) in Atlantic salmon (Salmo salar L.). HSMI is associated with Piscine orthoreovirus (PRV), and a search for a similar virus in the diseased rainbow trout led to detection of a sequence with 85% similarity to PRV. This finding called for a targeted effort to assess the risk the new PRV-variant pose on farmed rainbow trout and Atlantic salmon by studying infection and disease pathogenesis, aiming to provide more diagnostic knowledge. Based on the genetic relationship to PRV, the novel virus is referred to as PRV-Oncorhynchus mykiss (PRV-Om) in contrast to PRV-Salmo salar (PRV-Ss). In experimental trials, intraperitoneally injected PRV-Om was shown to replicate in blood in both salmonid species, but more effectively in rainbow trout. In rainbow trout, the virus levels peaked in blood and heart of cohabitants 6 weeks post challenge, along with increased expression of antiviral genes (Mx and viperin) in the spleen, with 80-100% of the cohabitants infected. Heart inflammation was diagnosed in all cohabitants examined 8 weeks post challenge. In contrast, less than 50% of the Atlantic salmon cohabitants were infected between 8 and 16 weeks post challenge and the antiviral response in these fish was very low. From 12 weeks post challenge and onwards, mild focal myocarditis was demonstrated in a few virus-positive salmon. In conclusion, PRV-Om infects both salmonid species, but faster transmission, more notable antiviral response and more prominent heart pathology were observed in rainbow trout.

Published

2017

36. A double-stranded probe coupled with isothermal amplification for qualitative and quantitative detection of avian reovirus.

Author

Kumar D, Chauhan TK, Agarwal RK, Dhama K, Goswami PP, Mariappan AK, Tiwari AK, and Mishra BP

Subjects

Animals, Chickens, DNA Primers genetics, Humans, Nucleic Acid Amplification Techniques instrumentation, Orthoreovirus, Avian classification, Orthoreovirus, Avian genetics, Polymerase Chain Reaction instrumentation, Polymerase Chain Reaction methods, Poultry Diseases diagnosis, Reoviridae Infections diagnosis, Reoviridae Infections virology, DNA, Viral genetics, Nucleic Acid Amplification Techniques methods, Orthoreovirus, Avian isolation & purification, Poultry Diseases virology, Reoviridae Infections veterinary

Abstract

We applied a probe-based real-time loop-mediated isothermal amplification (Cy5-RTqLAMP) technique targeting the avian reovirus (ARV) S3 gene to develop a rapid, sensitive, and specific method for virus detection and quantification. This test specifically detected the presence of ARV, but not other viruses or bacteria present in clinical or artificially spiked samples, including Newcastle disease virus, infectious bursal disease virus, fowl adenovirus, Marek's disease virus, Escherichia coli, and Salmonella spp. This test can detect ARV in less than one hour with an analytical sensitivity of 10 viral gene copies and 1 fg of total cDNA. The Cy5-RTqLAMP does not yield false positive results and is 100 times more sensitive than conventional PCR. This test was shown to be able to detect the presence of ARV in clinical samples. A similar strategy may be used for detection of other important human and animal viral pathogens.

Published

2017

37. Unusual clinical manifestations in Israeli ruminant populations infected with Orbiviruses.

Author

Bumbarov V, Golender N, Rotenberg D, and Brenner J

Subjects

Animals, Bluetongue diagnosis, Cattle, Hemorrhagic Disease Virus, Epizootic, Reoviridae Infections diagnosis, Ruminants, Sheep, Cattle Diseases diagnosis, Orbivirus, Reoviridae Infections veterinary, Sheep Diseases diagnosis

Abstract

Orbiviruses, some of which are virulent in ruminant species, are transmitted by blood- sucking insects. They can cause the smallest blood vessels to leak, leading to oedema, which is presented as Bluetongue (BT) and/or Epizootic haemorrhagic diseases (EHD). Other clinical manifestations include big-muscle necrosis, excessive scialorrea, and coronitis. Pathology and laboratory testing can con rm the involvement of orbivirus. Bluetongue infection in naïve sheep can elicit the 'classical signs' of the disease and, therefore, can warn of Bluetongue virus' (BTV) attacks and of increased vector activity. In 2006, infection of cattle by serotype 7 of the Epizootic haemorrhagic disease virus (EHDV) was detected in Israel, with lesions clinically identical to those of BT disease in sheep. In 2006, serotype 15 of the BTV (BTV-15) was isolated in Israel from sheep with acute BT. In 2008 clinical BT in cattle was reported and con rmed in Israel. To date, additional serotypes (BTV-2, BTV-4, BTV-5, BTV-8, BTV-12, BTV-16, and BTV-24) have been reported, of these BTV-5, BTV-8, BTV-12, and BTV-24 were isolated for the rst time in the region. Some of these serotypes have been detected in animals with simultaneous double/triple infections with di erent BTV serotypes, so that reassortment may also occur during these simultaneous infections. The use of local strains for the development of inactivated or subunit vaccines would however help to ensure antigenic matching. Various changes in orbiviral diseases occurred between 2006 and 2013 in Israel, and similarities and di erences between Israel and Europe have been reported in this study.

Published

2016

38. Confirmation of Elsey virus infection in a Queensland horse with mild neurologic signs.

Author

Agnihotri K, Pease B, Oakey J, and Campbell G

Subjects

Animals, Horse Diseases virology, Horses, Microscopy, Electron, Transmission veterinary, Orbivirus genetics, Phylogeny, Queensland, RNA, Viral genetics, Reoviridae Infections diagnosis, Reoviridae Infections virology, Sequence Analysis, RNA veterinary, Horse Diseases diagnosis, Orbivirus isolation & purification, Reoviridae Infections veterinary

Abstract

In 2011, a 2-year-old horse in northern Queensland, Australia, was reported to have developed mild neurologic signs, and a blood sample was submitted for laboratory investigation. Virus isolation was performed using the blood sample, and an orbivirus was isolated. This was confirmed to be a strain of Elsey virus (ELSV) after transmission electron microscopy and nucleotide sequencing. The nucleotide sequence was compared with those in GenBank, and had 100% identity with ELSV previously reported from the Northern Territory, Australia. ELSV is taxonomically closely related to Peruvian horse sickness virus., (© 2016 The Author(s).)

Published

2016

39. Serologic assays for the detection and strain identification of Pteropine orthoreovirus.

Author

Singh H, Shimojima M, Fukushi S, Fukuma A, Tani H, Yoshikawa T, Taniguchi S, Yang M, Sugamata M, Morikawa S, and Saijo M

Subjects

Animals, Antibodies, Viral blood, Communicable Diseases, Emerging immunology, Communicable Diseases, Emerging prevention & control, Communicable Diseases, Emerging virology, Enzyme-Linked Immunosorbent Assay, Genome, Viral, Hong Kong epidemiology, Humans, Indonesia epidemiology, Neutralization Tests methods, Orthoreovirus immunology, Orthoreovirus isolation & purification, Phylogeny, RNA, Viral, Rabbits, Reoviridae Infections virology, Respiratory Tract Infections diagnosis, Respiratory Tract Infections epidemiology, Respiratory Tract Infections prevention & control, Respiratory Tract Infections virology, Sequence Analysis, DNA, Viral Proteins immunology, Communicable Diseases, Emerging diagnosis, Orthoreovirus classification, Reoviridae Infections diagnosis, Reoviridae Infections prevention & control, Serologic Tests methods

Abstract

Pteropine orthoreovirus (PRV), potentially of bat origin, is reported to be a causative agent of emerging respiratory tract infections among humans in Southeast Asia. We evaluated the efficacy of serologic assays using the major outer capsid and cell attachment proteins (CAP) of PRV strains in the screening, confirmation and identification of three groups of human PRV infections; Indonesian/Japanese, Indonesian/Hong Kong and Malaysian strains. The different serologic assays were tested using rabbit polyclonal antisera raised against these proteins of selected PRV strains, and validation was carried out using sera from a Miyazaki-Bali/2007 PRV-infected patient and the patient's contacts. The results of this study showed that rabbit polyclonal antisera raised against the CAP of the Miyazaki-Bali/2007 PRV strain showed the highest reactivity to the Miyazaki-Bali/2007 PRV and to a lesser extent, cross-reactivity with the HK23629/07 and Melaka PRVs, respectively. Neutralization activity against the Miyazaki-Bali/2007 PRV was observed using rabbit anti-Miyazaki-Bali/2007 PRV CAP (320) but not with rabbit anti-HK23629/07 (<20) and Melaka (<20) PRV CAP. This lack of cross-neutralization, suggests the potential for human reinfection with different strains. The use of sera collected from contacts of the Miyazaki-Bali/2007 PRV-infected patient suggested that human-to-human infections with PRV are unlikely. Previously reported cases of PRV infections among human have been mild. However, the expanding geographic distribution of these viruses, of which its virulence remains unknown, warrants close monitoring to enable the development of prevention and control strategies in the event that a change in virulence occurs.

Published

2016

40. Whole genome alignment based one-step real-time RT-PCR for universal detection of avian orthoreoviruses of chicken, pheasant and turkey origins.

Author

Tang Y and Lu H

Subjects

Animals, Chickens virology, Genome, Viral, Genotype, RNA, Viral, Reproducibility of Results, Sensitivity and Specificity, Sequence Alignment, Turkeys virology, Galliformes virology, Orthoreovirus, Avian genetics, Poultry Diseases diagnosis, Reoviridae Infections diagnosis, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

Newly emerging avian orthoreovirus (ARV) variants have been continuously detected in Pennsylvania poultry since 2011. In this paper, we report our recent diagnostic assay development of one-step real-time RT-PCR (rRT-PCR) for the rapid and universal detection of all ARVs or reference strains of chicken, pheasant and turkey origins and six σC genotypes of the newly emerging field ARV variants in Pennsylvania (PA) poultry. Primers and probes for the rRT-PCR were designed from the conserved region of the M1 genome segment 5' end based on the whole-genome alignment of various ARV strains, including six field variants or novel strains obtained in PA poultry. The detection limit of the newly developed rRT-PCR for ARV was as low as 10 copies/reaction of viral RNA, and 10(0.50)-10(0.88) tissue culture infectious dose (TCID50)/100 μL of viruses. This new rRT-PCR detected all six σC genotypes from the 66 ARV field variant strains and reference strains tested in this study. There were no cross-reactions with other avian viruses. Reproducibility of the assay was confirmed by intra- and inter-assay tests with variability from 0.12% to 2.19%. Sensitivity and specificity of this new rRT-PCR for ARV were achieved at 100% and 88%, respectively, in comparison with virus isolation as the "gold standard" in testing poultry tissue specimen., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

41. Identification of novel viral infections of human concern provides continued opportunity for strengthening systemic public health capacity in Southeast Asia.

Author

Yano K

Subjects

Female, Humans, Male, Antibodies, Viral blood, Orthoreovirus immunology, Reoviridae Infections diagnosis

Published

2015

42. Serological evidence of human infection with Pteropine orthoreovirus in Central Vietnam.

Author

Singh H, Shimojima M, Ngoc TC, Quoc Huy NV, Chuong TX, Le Van A, Saijo M, Yang M, and Sugamata M

Subjects

Adolescent, Adult, Aged, Antibodies, Neutralizing blood, Enzyme-Linked Immunosorbent Assay, Female, Humans, Immunoglobulin G blood, Male, Middle Aged, Reoviridae Infections epidemiology, Serologic Tests, Vietnam epidemiology, Young Adult, Antibodies, Viral blood, Orthoreovirus immunology, Reoviridae Infections diagnosis

Abstract

Pteropine orthoreovirus, potentially of bat origin, has been reported to cause respiratory tract infections among human beings in Southeast Asia. Twelve IgG ELISA-positive cases with antibodies against Pteropine orthoreovirus were detected among 272 human serum samples collected between March and June 2014 from in and around Hue City, Central Vietnam. These 12 cases were IgM ELISA negative. Neutralizing antibodies were also detected among six of these cases with the highest titer of 1:1,280 in 2 cases (both female, 32 and 68 years old, respectively). This is the first report of human infection with Pteropine orthoreovirus in Central Vietnam. These findings indicate the need for surveillance on Pteropine orthoreovirus infections in Southeast Asia to enable prevention and control strategies to be developed should a change in virulence occur., (© 2015 Wiley Periodicals, Inc.)

Published

2015

43. Pteropine orthoreovirus infection among out-patients with acute upper respiratory tract infection in Malaysia.

Author

Voon K, Tan YF, Leong PP, Teng CL, Gunnasekaran R, Ujang K, Chua KB, and Wang LF

Subjects

Adolescent, Adult, Aged, Capsid Proteins genetics, Female, Genotype, Humans, Incidence, Malaysia epidemiology, Male, Middle Aged, Molecular Diagnostic Techniques, Oropharynx virology, Outpatients, Phylogeny, Reoviridae Infections epidemiology, Respiratory Tract Infections epidemiology, Sequence Analysis, DNA, Suburban Population, Young Adult, Orthoreovirus isolation & purification, Reoviridae Infections diagnosis, Respiratory Tract Infections virology

Abstract

This study aims to assess the incidence rate of Pteropine orthreovirus (PRV) infection in patients with acute upper respiratory tract infection (URTI) in a suburban setting in Malaysia, where bats are known to be present in the neighborhood. Using molecular detection of PRVs directly from oropharyngeal swabs, our study demonstrates that PRV is among one of the common causative agents of acute URTI with cough and sore throat as the commonest presenting clinical features. Phylogenetic analysis on partial major outer and inner capsid proteins shows that these PRV strains are closely related to Melaka and Kampar viruses previously isolated in Malaysia. Further study is required to determine the public health significance of PRV infection in Southeast Asia, especially in cases where co-infection with other pathogens may potentially lead to different clinical outcomes., (© 2015 Wiley Periodicals, Inc.)

Published

2015

44. Review of the 2012 Epizootic Hemorrhagic Disease Outbreak in Domestic Ruminants in the United States.

Author

Stevens G, McCluskey B, King A, O'Hearn E, and Mayr G

Subjects

Animal Diseases diagnosis, Animal Diseases epidemiology, Animals, Bison, Cattle, Deer, Disease Outbreaks statistics & numerical data, Geography, Hemorrhagic Disease Virus, Epizootic genetics, Host-Pathogen Interactions, Morbidity trends, RNA, Viral genetics, Reoviridae Infections diagnosis, Reoviridae Infections epidemiology, Reverse Transcriptase Polymerase Chain Reaction, Sheep, Time Factors, United States epidemiology, Animal Diseases virology, Animals, Domestic virology, Disease Outbreaks veterinary, Hemorrhagic Disease Virus, Epizootic physiology, Reoviridae Infections veterinary, Ruminants virology

Abstract

An unusually large number of cases of Epizootic hemorrhagic disease (EHD) were observed in United States cattle and white-tailed deer in the summer and fall of 2012. USDA APHIS Veterinary Services area offices were asked to report on foreign animal disease investigations and state diagnostic laboratory submissions which resulted in a diagnosis of EHD based on positive PCR results. EHD was reported in the following species: cattle (129 herds), captive white-tailed deer (65 herds), bison (8 herds), yak (6 herds), elk (1 herd), and sheep (1 flock). A majority of the cases in cattle and bison were found in Nebraska, South Dakota, and Iowa. The majority of cases in captive white-tailed deer were found in Ohio, Iowa, Michigan, and Missouri. The most common clinical sign observed in the cattle and bison herds was oral lesions. The major observation in captive white-tailed deer herds was death. Average within-herd morbidity was 7% in cattle and bison herds, and 46% in captive white-tailed deer herds. The average within-herd mortality in captive white-tailed deer herds was 42%.

Published

2015

45. Development and application of molecular methods (PCR) for detection of Tasmanian Atlantic salmon reovirus.

Author

Zainathan SC, Carlile G, Carson J, McColl KA, Crane MS, Williams LM, Hoad J, Moody NJ, Aiken HM, Browning GF, and Nowak BF

Subjects

Animals, Cell Line, Fish Diseases epidemiology, Fish Diseases virology, Molecular Sequence Data, Prevalence, Reoviridae genetics, Reoviridae Infections diagnosis, Reoviridae Infections epidemiology, Reoviridae Infections virology, Salmo salar virology, Sensitivity and Specificity, Tasmania, Aquaculture methods, Fish Diseases diagnosis, Polymerase Chain Reaction veterinary, Reoviridae physiology, Reoviridae Infections veterinary

Abstract

Molecular (PCR) diagnostic tests for the detection and identification of aquareovirus in general, and Tasmanian Atlantic salmon reovirus (TSRV) specifically, were developed, and their diagnostic sensitivity and specificity were determined and compared with virus isolation in cell culture. Intralaboratory and interlaboratory comparison of PCR (conventional hemi-nested RT-PCR & RT-qPCR) and virus isolation in cell culture using finfish cell lines, CHSE-214 and EPC, was carried out for the detection and identification of TSRV using field samples of farmed Atlantic salmon Salmo salar, L. from various aquaculture sites around Tasmania. The interlaboratory comparison of diagnostic methods was carried out between two laboratories, AAHL-CSIRO and DPIPWE-Tasmania. A total of 144 fish from nine sites (12-33 fish per site) were sampled from two regions of Tasmania (Tamar River estuary in the north and Huon River estuary in the south-east) during late spring to early summer of 2009, and the data were analysed using different statistical approaches. The prevalence of TSRV ranged from 6% to 22% in both regions. All the diagnostic methods (data from both laboratories) had high specificity, while the estimated sensitivity varied between tests with RT-qPCR being the most sensitive (95.2%) method followed by virus isolation and then conventional hemi-nested RT-PCR., (© 2014 John Wiley & Sons Ltd.)

Published

2015

46. Development and application of an indirect ELISA for the detection of antibodies to novel duck reovirus.

Author

Yun T, Chen H, Yu B, Zhang C, Chen L, Ni Z, Hua J, and Ye W

Subjects

Animals, Antigens, Viral immunology, Bird Diseases virology, Capsid Proteins immunology, China epidemiology, Reoviridae Infections diagnosis, Reoviridae Infections virology, Sensitivity and Specificity, Seroepidemiologic Studies, Antibodies, Viral blood, Bird Diseases diagnosis, Ducks virology, Enzyme-Linked Immunosorbent Assay methods, Orthoreovirus, Avian immunology, Reoviridae Infections veterinary, Veterinary Medicine methods

Abstract

A novel duck reovirus (N-DRV) disease emerged in China in 2000 and it has become an epidemic genotype. A test for detection of virus-specific antibodies in serum samples would be useful for epidemiological investigations. Currently, Currently, serological assays for N-DRV diagnosis are not available. A test for detection of virus-specific antibodies in serum samples would be useful for epidemiological investigations. In this study, a highly sensitive and specific indirect enzyme-linked immunosorbent assay (ELISA) for the detection of antibodies to N-DRV was developed. The outer capsid (σC) of N-DRV was cloned and expressed in Escherichia coli as a coating antigen. The antigen concentration and serum dilution were optimized using a checkerboard titration. Furthermore, the specificity of σC-ELISA assay was confirmed by cross checking with other duck viral pathogens. In comparison with the western blot, the sensitivity and specificity of the σC-ELISA was 92.6% and 88.9%, respectively, and agreement of two tests was excellent with κ value of 0.786 (p < 0.05). A serological survey was performed using the assay on serum samples from different age and species of duck flocks in the Zhejiang and Jiangsu Province, China. The seropositive rate of the 1209 serum samples was 57.7%. In conclusion, the developed σC-ELISA assay is a very specific and sensitive test that will be useful for large-scale serological survey in N-DRV infection and monitoring antibodies titers against N-DRV., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

47. Evidence for viral infection as a causative factor of human biliary atresia.

Author

Saito T, Terui K, Mitsunaga T, Nakata M, Ono S, Mise N, and Yoshida H

Subjects

Humans, Polymerase Chain Reaction, Reoviridae Infections complications, Reoviridae Infections diagnosis, Virus Diseases diagnosis, Biliary Atresia virology, Virus Diseases complications

Abstract

Objectives: To explore the evidence for viral infections triggering human biliary atresia (BA) by reviewing archival original articles that analyzed human samples via polymerase chain reaction (PCR) experiments, considering the recent experimental trend of extensive use of rotaviral BA animal models., Methods: A PubMed search retrieved original articles that reported the results of PCR experiments for detecting viral DNA or RNA in patient samples as proof of past infection. Search terms included the often-debated DNA or RNA viruses and BA. Special focus was directed toward PCR analyses that targeted reovirus and rotavirus, where PCR accuracy, specimen characteristics and their interpretations were compared., Results: Nineteen studies were conducted on 16 different kinds of viruses using PCR, with 5 studies on reovirus, 3 on rotavirus, 10 on cytomegalovirus, 5 on Epstein-Barr virus, 4 on parvovirus B19, and so on. Among the papers suggesting a possible viral link to only BA, there was no study on reovirus, 1 on rotavirus, 3 on cytomegalovirus, 1 on EB virus, and 1 on papillomavirus. Of the 6 PCR studies on Reoviridae, 3 on reovirus and 2 on rotavirus were evaluated rigorously for experimental accuracy, including their sensitivity. Two research groups analyzed preoperative stool samples in addition to generic hepatobiliary tissue obtained at surgery. Sample collection timing varied widely, with storage period prior to PCR experimentation not revealed in most reports on Reoviridae., Conclusion: Although a considerable number of PCR studies have sought to clarify a viral role in the pathogenesis of BA using human samples, the findings have been contradictory and have not succeeded in achieving an obvious differentiation between causative and accidental infection of the focused virus. Reproducible and convincing evidence for a causative Reoviridae infection has been lacking based on objective data from highly sensitive PCR experiments. Even though the possibility remains of viral disappearance at the timing of collection, to avoid further ambiguous interpretations of PCR results, rigorous and meticulous collection of large numbers of specimens at carefully planned timing, along with a strictly adjusted and finely tuned PCR system, is strongly recommended for obtaining more reliable and consistent results., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

48. Orbiviruses: A Gap Analysis.

Author

Gay CG

Subjects

Animals, Bluetongue diagnosis, Bluetongue epidemiology, Bluetongue prevention & control, Bluetongue virus immunology, Disease Outbreaks prevention & control, Hemorrhagic Disease Virus, Epizootic immunology, Humans, Livestock, Reoviridae Infections diagnosis, Reoviridae Infections epidemiology, Sheep, Orbivirus immunology, Reoviridae Infections prevention & control

Published

2015

49. Diagnostic Tools for Bluetongue and Epizootic Hemorrhagic Disease Viruses Applicable to North American Veterinary Diagnosticians.

Author

Wilson WC, Daniels P, Ostlund EN, Johnson DE, Oberst RD, Hairgrove TB, Mediger J, and McIntosh MT

Subjects

Animals, Bluetongue virus genetics, Bluetongue virus immunology, Genotype, Hemorrhagic Disease Virus, Epizootic genetics, Hemorrhagic Disease Virus, Epizootic immunology, High-Throughput Nucleotide Sequencing veterinary, North America, Reoviridae Infections diagnosis, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Sheep, Bluetongue diagnosis, Bluetongue virus isolation & purification, Genotyping Techniques veterinary, Hemorrhagic Disease Virus, Epizootic isolation & purification, Reoviridae Infections veterinary

Abstract

This review provides an overview of current and potential new diagnostic tests for bluetongue (BT) and epizootic hemorrhagic disease (EHD) viruses compiled from international participants of the Orbivirus Gap Analysis Workshop, Diagnostic Group. The emphasis of this review is on diagnostic tools available to North American veterinary diagnosticians. Standard diagnostic tests are readily available for BT/EHD viruses, and there are described tests that are published in the World Organization for Animal Health (OIE) Terrestrial Manual. There is however considerable variation in the diagnostic approach to these viruses. Serological assays are well established, and many laboratories are experienced in running these assays. Numerous nucleic acid amplification assays are also available for BT virus (BTV) and EHD virus (EHDV). Although there is considerable experience with BTV reverse-transcriptase PCR (RT-PCR), there are no standards or comparisons of the protocols used by various state and federal veterinary diagnostic laboratories. Methods for genotyping BTV and EHDV isolates are available and are valuable tools for monitoring and analyzing circulating viruses. These methods include RT-PCR panels or arrays, RT-PCR and sequencing of specific genome segments, or the use of next-generation sequencing. In addition to enabling virus characterization, use of advanced molecular detection methods, including DNA microarrays and next-generation sequencing, significantly enhance the ability to detect unique virus strains that may arise through genetic drift, recombination, or viral genome segment reassortment, as well as incursions of new virus strains from other geographical areas.

Published

2015

50. Epizootic hemorrhagic disease in a yak.

Author

Raabis SM, Byers SR, Han S, and Callan RJ

Subjects

Animals, Cattle, Cattle Diseases pathology, Cattle Diseases virology, Male, Reoviridae Infections diagnosis, Reoviridae Infections pathology, Reoviridae Infections virology, Cattle Diseases diagnosis, Hemorrhagic Disease Virus, Epizootic, Reoviridae Infections veterinary

Abstract

Epizootic hemorrhagic disease virus (EHDV) infection was diagnosed in a 3-year-old yak. The yak had signs of intermittent tremors, dysphagia, oral ulcerative lesions, hemorrhagic enteritis, tachypnea, and thrombocytopenia. Postmortem diagnostics confirmed EHDV (serotype 2) using reverse-transcriptase polymerase chain reaction (RT-PCR). Gross and histopathological results were consistent with EHDV reported in other species.

Published

2014