Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep

Detalhes bibliográficos
Autor(a) principal: de Moraes, Érica Paes Barreto Xavier
Data de Publicação: 2013
Outros Autores: de Freitas, Antônio Carlos, da Costa, Mateus Matiuzzi, Júnior, José Wilton Pinheiro, Mota, Rinaldo Aparecido
Tipo de documento: Artigo
Idioma: por
Título da fonte: Brazilian Journal of Veterinary Medicine
Texto Completo: https://rbmv.org/BJVM/article/view/637
Resumo: ABSTRACT. de Moraes E.P.B.X., Freitas A.C., Costa M.M., PinheiroJr J.W. & Mota R.A. [Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep]. Utilização da PCR nested para detecção de Toxoplasma gondii no sangue de ovelhas experimentalmente infectadas. Revista Brasileira de Medicina Veterinária, 35(4):329-334, 2013. Laboratório de Doenças Infecto-Contagiosas dos Animais Domésticos, Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Rua Dom Manoel de Medeiros, s/n, Dois Irmãos, Recife, PE 52171-900, Brasil. E-mail: ericaxmoraes@globo.com The aim of this study was to evaluate the sensitivity of the PCR and nested PCR for T. gondii detection in the blood of experimentally infected sheep with tachyzoites through the semen. Blood samples of 41 sheep were taken, which were infected with different dosages: G1 - 6.5 X 104 tachyzoites; G2- 4 X 107 tachyzoites and G3- control group. For the anti-T.gondii antibodies research the Indirect Immunofluorescence (IIF) technique was used. For the PCR and nested PCR, primers derived from B1 gene were used. Seroconversion was observed only for the infected group. In the PCR, T. gondii DNA was detected in 40% of the infected sheep blood samples, and in the nested PCR, in 93.3% of the samples. In the G3, no antibodies were detected, as well as parasitic DNA in neither of the animals. It is possible to conclude that the nested PCR is more sensitive for the T. gondii detection in the blood of animals experimentally infected through the semen, presenting superior results in comparison to those of the PCR and might be successfully used in studies like this one.
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spelling Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheepUTILIZAÇÃO DA PCR NESTED PARA DETECÇÃO DE Toxoplasma gondii NO SANGUE DE OVELHAS EXPERIMENTALMENTE INFECTADASDiagnósticotoxoplasmose ovinatécnica molecularDiagnosetoxoplasmosis in sheepmolecular techniqueABSTRACT. de Moraes E.P.B.X., Freitas A.C., Costa M.M., PinheiroJr J.W. & Mota R.A. [Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep]. Utilização da PCR nested para detecção de Toxoplasma gondii no sangue de ovelhas experimentalmente infectadas. Revista Brasileira de Medicina Veterinária, 35(4):329-334, 2013. Laboratório de Doenças Infecto-Contagiosas dos Animais Domésticos, Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Rua Dom Manoel de Medeiros, s/n, Dois Irmãos, Recife, PE 52171-900, Brasil. E-mail: ericaxmoraes@globo.com The aim of this study was to evaluate the sensitivity of the PCR and nested PCR for T. gondii detection in the blood of experimentally infected sheep with tachyzoites through the semen. Blood samples of 41 sheep were taken, which were infected with different dosages: G1 - 6.5 X 104 tachyzoites; G2- 4 X 107 tachyzoites and G3- control group. For the anti-T.gondii antibodies research the Indirect Immunofluorescence (IIF) technique was used. For the PCR and nested PCR, primers derived from B1 gene were used. Seroconversion was observed only for the infected group. In the PCR, T. gondii DNA was detected in 40% of the infected sheep blood samples, and in the nested PCR, in 93.3% of the samples. In the G3, no antibodies were detected, as well as parasitic DNA in neither of the animals. It is possible to conclude that the nested PCR is more sensitive for the T. gondii detection in the blood of animals experimentally infected through the semen, presenting superior results in comparison to those of the PCR and might be successfully used in studies like this one.Objetivou-se com esse estudo avaliar a sensibilidade da PCR e PCR nested na detecção de T. gondiino sangue de ovelhas experimentalmente infectadas com taquizoítos via sêmen. Foram colhidas amostras de sangue de 30 ovelhas infectadas com diferentes doses: G1- 6,5 X 104 taquizoítos; G2- 4 X 107 taquizoítos e G3- grupo controle. Para a pesquisa de anticorpos anti-T. gondii foi utilizada a técnica de Imunofluorescência Indireta (IFI). Para o PCR e PCR nested foram utilizados iniciadores derivados do gene B1. Observou-se soroconversão apenas dos grupos infectados. Na PCR, detectou-se o DNA do T. gondii em 40% e na PCR nested em 93,3% amostras de sangue das ovelhas infectadas. No G3 não foi detectado anticorpos e DNA parasitário em nenhum animal.Conclui-se que a PCR nested é mais sensível na detecção de T. gondii no sangue de animais experimentalmente infectados via sêmen, mostrando resultado superior ao da PCR e podendo ser utilizada com êxito em estudos dessa natureza.Sociedade de Medicina Veterinária do Estado do Rio de Janeiro.2013-12-15info:eu-repo/semantics/articleinfo:eu-repo/semantics/publishedVersionpeer reviewedAvaliado pelos paresapplication/pdfhttps://rbmv.org/BJVM/article/view/637Brazilian Journal of Veterinary Medicine; Vol. 35 No. 4 (2013); 329-334Revista Brasileira de Medicina Veterinária; v. 35 n. 4 (2013); 329-3342527-21790100-2430reponame:Brazilian Journal of Veterinary Medicineinstname:Sociedade de Medicina Veterinária do Estado do Rio de Janeiro (SOMVERJ)instacron:SBMVporhttps://rbmv.org/BJVM/article/view/637/502de Moraes, Érica Paes Barreto Xavierde Freitas, Antônio Carlosda Costa, Mateus MatiuzziJúnior, José Wilton PinheiroMota, Rinaldo Aparecidoinfo:eu-repo/semantics/openAccess2020-12-23T17:30:52Zoai:ojs.rbmv.org:article/637Revistahttps://rbmv.org/BJVMONGhttps://rbmv.org/BJVM/oaicontato.rbmv@gmail.com2527-21790100-2430opendoar:2020-12-23T17:30:52Brazilian Journal of Veterinary Medicine - Sociedade de Medicina Veterinária do Estado do Rio de Janeiro (SOMVERJ)false
dc.title.none.fl_str_mv Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
UTILIZAÇÃO DA PCR NESTED PARA DETECÇÃO DE Toxoplasma gondii NO SANGUE DE OVELHAS EXPERIMENTALMENTE INFECTADAS
title Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
spellingShingle Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
de Moraes, Érica Paes Barreto Xavier
Diagnóstico
toxoplasmose ovina
técnica molecular
Diagnose
toxoplasmosis in sheep
molecular technique
title_short Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
title_full Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
title_fullStr Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
title_full_unstemmed Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
title_sort Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep
author de Moraes, Érica Paes Barreto Xavier
author_facet de Moraes, Érica Paes Barreto Xavier
de Freitas, Antônio Carlos
da Costa, Mateus Matiuzzi
Júnior, José Wilton Pinheiro
Mota, Rinaldo Aparecido
author_role author
author2 de Freitas, Antônio Carlos
da Costa, Mateus Matiuzzi
Júnior, José Wilton Pinheiro
Mota, Rinaldo Aparecido
author2_role author
author
author
author
dc.contributor.author.fl_str_mv de Moraes, Érica Paes Barreto Xavier
de Freitas, Antônio Carlos
da Costa, Mateus Matiuzzi
Júnior, José Wilton Pinheiro
Mota, Rinaldo Aparecido
dc.subject.por.fl_str_mv Diagnóstico
toxoplasmose ovina
técnica molecular
Diagnose
toxoplasmosis in sheep
molecular technique
topic Diagnóstico
toxoplasmose ovina
técnica molecular
Diagnose
toxoplasmosis in sheep
molecular technique
description ABSTRACT. de Moraes E.P.B.X., Freitas A.C., Costa M.M., PinheiroJr J.W. & Mota R.A. [Nested PCR utilization for Toxoplasma gondii detection in the blood of experimentally infected sheep]. Utilização da PCR nested para detecção de Toxoplasma gondii no sangue de ovelhas experimentalmente infectadas. Revista Brasileira de Medicina Veterinária, 35(4):329-334, 2013. Laboratório de Doenças Infecto-Contagiosas dos Animais Domésticos, Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Rua Dom Manoel de Medeiros, s/n, Dois Irmãos, Recife, PE 52171-900, Brasil. E-mail: ericaxmoraes@globo.com The aim of this study was to evaluate the sensitivity of the PCR and nested PCR for T. gondii detection in the blood of experimentally infected sheep with tachyzoites through the semen. Blood samples of 41 sheep were taken, which were infected with different dosages: G1 - 6.5 X 104 tachyzoites; G2- 4 X 107 tachyzoites and G3- control group. For the anti-T.gondii antibodies research the Indirect Immunofluorescence (IIF) technique was used. For the PCR and nested PCR, primers derived from B1 gene were used. Seroconversion was observed only for the infected group. In the PCR, T. gondii DNA was detected in 40% of the infected sheep blood samples, and in the nested PCR, in 93.3% of the samples. In the G3, no antibodies were detected, as well as parasitic DNA in neither of the animals. It is possible to conclude that the nested PCR is more sensitive for the T. gondii detection in the blood of animals experimentally infected through the semen, presenting superior results in comparison to those of the PCR and might be successfully used in studies like this one.
publishDate 2013
dc.date.none.fl_str_mv 2013-12-15
dc.type.driver.fl_str_mv info:eu-repo/semantics/article
info:eu-repo/semantics/publishedVersion
peer reviewed
Avaliado pelos pares
format article
status_str publishedVersion
dc.identifier.uri.fl_str_mv https://rbmv.org/BJVM/article/view/637
url https://rbmv.org/BJVM/article/view/637
dc.language.iso.fl_str_mv por
language por
dc.relation.none.fl_str_mv https://rbmv.org/BJVM/article/view/637/502
dc.rights.driver.fl_str_mv info:eu-repo/semantics/openAccess
eu_rights_str_mv openAccess
dc.format.none.fl_str_mv application/pdf
dc.publisher.none.fl_str_mv Sociedade de Medicina Veterinária do Estado do Rio de Janeiro.
publisher.none.fl_str_mv Sociedade de Medicina Veterinária do Estado do Rio de Janeiro.
dc.source.none.fl_str_mv Brazilian Journal of Veterinary Medicine; Vol. 35 No. 4 (2013); 329-334
Revista Brasileira de Medicina Veterinária; v. 35 n. 4 (2013); 329-334
2527-2179
0100-2430
reponame:Brazilian Journal of Veterinary Medicine
instname:Sociedade de Medicina Veterinária do Estado do Rio de Janeiro (SOMVERJ)
instacron:SBMV
instname_str Sociedade de Medicina Veterinária do Estado do Rio de Janeiro (SOMVERJ)
instacron_str SBMV
institution SBMV
reponame_str Brazilian Journal of Veterinary Medicine
collection Brazilian Journal of Veterinary Medicine
repository.name.fl_str_mv Brazilian Journal of Veterinary Medicine - Sociedade de Medicina Veterinária do Estado do Rio de Janeiro (SOMVERJ)
repository.mail.fl_str_mv contato.rbmv@gmail.com
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