Evaluation of an alternative indirect-ELISA test using in vitro-propagated Trypanosoma brucei brucei whole cell lysate as antigen for the detection of anti-Trypanosoma evansi IgG in Colombian livestock

Surra is a zoonotic disease caused by Trypanosoma evansi, affecting the health and production of the livestock significantly. There are several methods to diagnose this disease, which have different principles, sensitivity, and specificity. Among them, the serological techniques using T. evansi as a...

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Autores:
Jaimes Dueñez, Jeiczon Elim
Zapata-Zapata C.
Triana-Chávez O.
Mejía-Jaramillo A.M.
Tipo de recurso:
Article of journal
Fecha de publicación:
2019
Institución:
Universidad Cooperativa de Colombia
Repositorio:
Repositorio UCC
Idioma:
OAI Identifier:
oai:repository.ucc.edu.co:20.500.12494/41567
Acceso en línea:
https://doi.org/10.1089/aid.2011.0297
https://www.scopus.com/inward/record.uri?eid=2-s2.0-85059014212&doi=10.2147%2fPRBM.S165816&partnerID=40&md5=bc932af380963a63be14379df26e83ab
https://hdl.handle.net/20.500.12494/41567
Palabra clave:
genomic DNA
immunoglobulin G
immunoglobulin G
parasite antigen
agar gel electrophoresis
Anaplasma marginale
antibody detection
antigen detection
Article
Babesia bigemina
Babesia bovis
cell lysate
Colombian
controlled study
cross reaction
enzyme linked immunosorbent assay
in vitro study
livestock
molecular diagnosis
nonhuman
priority journal
sensitivity and specificity
surra
taurine cattle
Tetranychus evansi
Trypanosoma brucei brucei
Trypanosoma evansi
Trypanosoma vivax
whole cell
animal
bovine
Colombia
comparative study
enzyme linked immunosorbent assay
evaluation study
isolation and purification
livestock
polymerase chain reaction
procedures
Trypanosoma brucei brucei
veterinary medicine
Animals
Antigens
Protozoan
Cattle
Colombia
Enzyme-Linked Immunosorbent Assay
Immunoglobulin G
Livestock
Polymerase Chain Reaction
Trypanosoma brucei brucei
Rights
closedAccess
License
http://purl.org/coar/access_right/c_14cb
Description
Summary:Surra is a zoonotic disease caused by Trypanosoma evansi, affecting the health and production of the livestock significantly. There are several methods to diagnose this disease, which have different principles, sensitivity, and specificity. Among them, the serological techniques using T. evansi as antigen are powerful tools for its epidemiological surveillance. However, they are poorly used due to inefficient in vitro propagation of T. evansi, which requires the use of laboratory animals for antigen production. In the present study, whole cell lysate of T. brucei brucei propagated in vitro was used as an antigen for the detection of anti-T. evansi immunoglobulin G in cattle through an indirect-ELISA. Based on a total of 45 samples from non-infected and 45 samples from T. evansi infected cattle, the sensitivity and specificity were estimated as 100% and 97.7%, respectively. After the validation, serological and molecular surveys were carried out in 710 cattle samples from two endemic Colombian regions (Antioquia and Arauca departments) for T. evansi where molecular prevalences of ˜7.0% were detected through the year and sporadic outbreaks of T. vivax infections have been associated to low prevalence of this species (<1%). A total of 424 (59.7%) samples were positive by indirect-ELISA T. b. brucei, while PCR test for T. evansi and T. vivax, showed 49 (6.9%) and no positive samples, respectively. Interestingly, categories of animals aged>1 year, Bos taurus breed, and those raised under intensive farming system exhibited a higher seroprevalence to T. evansi (P < 0.05). The results displayed a new alternative for antibody detection anti-T. evansi in livestock, using parasites propagated in vitro as antigen, which presents the advantage of higher standardization potential, and avoid the use of live animal for antigen production. A larger availability of this ELISA will generate useful information for a better understanding of the epidemiologic aspects, as well as for the management and control of these diseases in Colombia. However, the ability of the test to detect and/or cross react with T. vivax infections remains to be investigated. © 2019

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