Validation of an immunoblot assay employing an objective reading system and used as a confirmatory test in equine infectious anaemia surveillance programs.
Abstract: Equine infectious anaemia (EIA) is a blood borne disease that is listed among the notifiable diseases of the World Organisation for Animal Health (OIE). EIA is also regulated by the OIE for the international trading provisions and is generally subject to control programmes. Since 2011, Italy has been conducting a surveillance plan based on a three-tier diagnostic system, using a serological ELISA as screening test, an agar gel immunodiffusion test (AGIDT) as a confirmatory method, and an immunoblot (IB) as an alternative confirmatory assay for discordant results between the first two tests. As for the in-house competitive ELISA (c-ELISA) and the AGIDT, the Italian National Reference Laboratory for EIA (NRL) validated the IB according to the OIE guidelines, employing eight panels containing positive sera, including those from EIA virus (EIAV) proven infected horses, and negative horse, mule and donkey sera collected from different geographical areas. In addition, two international reference image panels were employed for the optimization and the validation of the digital image reading system adopted that allows an impartial measurement of the serum reactivity in the IB assay. The immunological reactivity to EIAV antigens, p26, gp45 and gp90 adsorbed on the IB membrane, determines the serological status of the animal and for EIA, a p26 positive band together with at least one of the other antigen defines a subject as serologically positive for EIAV. For validation, the parameters assessed were threshold values, analytical and diagnostic sensitivity and specificity, repeatability and reproducibility. These parameters were evaluated for each antigen as well as in combination, according to the diagnostic algorithm established above. The validation data defined the IB as having a satisfactory sensitivity, specificity, repeatability and reproducibility for all antigens and species tested. An instrumental recording of the results improves the confidence in using IB as a confirmatory test for EIAV, differently from the AGIDT that is read by an operator. The advantages of using the IB are its higher sensitivity, to that of the AGIDT, which allows an earlier detection of infection that reduces the risk of transmission and therefore the incidence of the EIA, and its higher specificity to that of the ELISA which is based on the discrimination of subjects reacting only against the p26, the antigen used by all ELISAs available, which are not considered as infected by EIAV. In particular, when this assay is used in outbreaks it can detect new cases earlier than the AGIDT, and therefore reduce the restriction period with an economic benefit for the animal owners and the public veterinary sanitary system.
Copyright © 2019. Published by Elsevier B.V.
Publication Date: 2019-01-23 PubMed ID: 30684508DOI: 10.1016/j.jviromet.2019.01.012Google Scholar: Lookup
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- Journal Article
- Research Support
- Non-U.S. Gov't
- Validation Study
- Antibodies
- Antigen
- Diagnosis
- Diagnostic Technique
- Disease control
- Disease Diagnosis
- Disease Outbreaks
- Disease Prevention
- Disease Surveillance
- Disease Treatment
- Epidemiology
- Equine Health
- Equine Infectious Anemia
- Immunoblotting
- Immunology
- Infectious Disease
- Public Health
- Serology
- Veterinary Medicine
- Veterinary Procedure
- Veterinary Research
Summary
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The research validates an immunoblot (IB) assay, used to detect antibodies related to equine infectious anaemia (EIA) in horses, mules, and donkeys. This assay is used as a confirmatory test in surveillance programs designed to control the spread of this disease, with results indicating it has satisfactory sensitivity, specificity, repeatability and reproducibility.
Background of the Research
- EIA is a major worldwide disease that affects equines such as horses, mules, and donkeys. It’s regulated internationally, and Italy has implemented a three-tier diagnostic system to monitor and control the disease.
- The diagnostic system includes an initial screening ELISA (Enzyme-Linked Immunosorbent Assay), followed by a confirmatory AGIDT (Agar Gel Immunodiffusion Test) and if there are conflicting results between these two, an immunoblot (IB) assay is used as the final step for confirmation.
Methodology of the Validation
- IB was validated by the Italian National Reference Laboratory for EIA in line with global standards. The assay was tested using positive sera from known infected equines and negative sera from different geographic regions.
- Additionally, international reference image panels were used for further validation and optimization of the digital image reading system used in the assay. This system allows for an objective evaluation of the serum reactivity in the IB assay.
Findings of the Validation
- The validation process defined certain parameters such as threshold values, analytical and diagnostic sensitivity and specificity, as well as reproducibility. Each antigen, as well as their combination, was evaluated according to a set diagnostic algorithm.
- A successful validation resulted in the IB assay demonstrating satisfactory sensitivity, specificity, repeatability, and reproducibility across the different species and for all antigens tested.
Significance and Implications
- The use of an instrumental system ensures objectivity and boosts confidence in the use of IB as a confirmatory test, as compared to the manually-read AGIDT.
- The improved sensitivity of the IB assay over the AGIDT means potential early detection of EIA and therefore reducing the risk and spread of this disease.
- The specificity of the IB assay is also greater than that of the ELISA which can lead to less false positives.
- If used during EIA outbreaks, this test could potentially reduce restrictions faster, yielding economic benefits for animal owners and the public veterinary health system.
Cite This Article
APA
(2019).
Validation of an immunoblot assay employing an objective reading system and used as a confirmatory test in equine infectious anaemia surveillance programs.
J Virol Methods, 266, 77-88.
https://doi.org/10.1016/j.jviromet.2019.01.012 Publication
Researcher Affiliations
MeSH Terms
- Animals
- Antibodies, Viral / blood
- Enzyme-Linked Immunosorbent Assay
- Epidemiological Monitoring / veterinary
- Equine Infectious Anemia / blood
- Equine Infectious Anemia / diagnosis
- Horses / virology
- Image Processing, Computer-Assisted
- Immunoblotting / standards
- Infectious Anemia Virus, Equine / immunology
- Italy
- Reproducibility of Results
- Sensitivity and Specificity
Citations
This article has been cited 3 times.- Ostuni A, Frontoso R, Crudele MA, Barca L, Amati M, Boni R, De Vendel J, Raimondi P, Bavoso A. Comparative Evaluation of a Multistrain Indirect ELISA Targeting Anti- p26 and gp45 Antibodies for EIAV Detection. Pathogens 2025 Jun 8;14(6).
- Carvelli A, Nardini R, Carnio A, Ricci I, Rosone F, Sala M, Simeoni S, Maccarone D, Scicluna MT. Equine Infectious Anaemia: The Active Surveillance of an Entire Equid Population Reduces the Occurrence of the Infection. Transbound Emerg Dis 2024;2024:3439871.
- Cardeti G, Manna G, Cersini A, Nardini R, Rosati S, Reina R, Cittadini M, Sittinieri S, Altigeri A, Marcario GA, Scicluna MT. Horse Innate Immunity in the Control of Equine Infectious Anemia Virus Infection: A Preliminary Study. Viruses 2024 Nov 21;16(12).
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