Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos

Andreolla, Ana Paula

Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos

Detalhes bibliográficos
Autor(a) principal:	Andreolla, Ana Paula
Data de Publicação:	2017
Tipo de documento:	Dissertação
Idioma:	por
Título da fonte:	Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF)
Texto Completo:	http://tede.upf.br/jspui/handle/tede/1590
Resumo:	Bovine Leukemia Virus (BLV) is the etiological agent of enzootic bovine leukemia (EBL) a persistent infectious disease highly prevalent in dairy cattle. Serological testing and culling infected animals are central to disease control. The agar gel immunodiffusion (AGID) assay that uses BLV cultivated in Fetal Lamb Kidney cells is the only assay produced in Brazil and used in most laboratories for EBL diagnosis. Aiming to fulfil this gap, we developed an indirect ELISA based on the recombinant capsid protein (p24) of BLV to detect antibodies in cattle. To reach our goals, we designed PCR primers to amplify the nucleotides coding for the p24 protein and cloned the resulting DNA fragment in the pET-20 plasmid. The resulting plasmid was transformed in competent E. coli ER2566 and the protein expression was induced by IPTG (0.1mM). The protein (BLVp24r) was purified using a HisTrap column coupled to an ÄKTA Pure Chromatography equipment, and later analyzed by SDS-PAGE. The antigenicity and immunogenicity of the BLVp24r were evaluated by Western blot using sera from rats immunized with BLVrp24 and with sera from naturally infected cows prior to the development of the ELISA. For the ELISA, the microplate type, antigen concentration and serum dilution were determined by checkboard analysis. The receptor operation characteristics (ROC) curve analysis and the area under the curve (AUC) analysis were used to evaluate the ELISA performance. After that, the ELISA was used to evaluate the prevalence of anti-BLV antibodies in cattle blood. The BLVp24r protein was expressed as a fusion protein and had a molecular mass of 67 KDa. Only the serum from immunized rats and from cattle naturally infected with BLV recognized the BLVp24r by Western blot. The PolySorp® plates provide the bestperformance on the BLVp24r ELISA with 50 ng/well of the protein and with bovine serum diluted 1:100. Our indirect ELISA to BLV was set with a cut-off value of 0.320 at OD450nm and had sensibility of 98.5% and 100% specificity. The ROC had an AUC value of 0.9989 (95% confidence interval from 0.9961 to 1.002), indicating high level of precision. With this ELISA we screened sera samples from cattle and found a prevalence of antibodies to BLV in 31.1% of dairy cattle and 9.5% in beef cattle. The BLVp24r is suitable to detect antibodies to BLV in bovine serum by ELISA and should be a strong candidate for the development of a commercial assay aimingto control EBL in cattle.

Metadados do item

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spelling	Kreutz, Luiz Carlos56057555953http://lattes.cnpq.br/620709094409282001947247000http://lattes.cnpq.br/5525234743711148Andreolla, Ana Paula2018-12-18T19:24:52Z2017-08-07ANDREOLLA, Ana Paula. Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos. 2017. 49 f. Dissertação (Mestrado em Bioexperimentação) - Universidade de Passo Fundo, Passo Fundo, RS, 2017.http://tede.upf.br/jspui/handle/tede/1590Bovine Leukemia Virus (BLV) is the etiological agent of enzootic bovine leukemia (EBL) a persistent infectious disease highly prevalent in dairy cattle. Serological testing and culling infected animals are central to disease control. The agar gel immunodiffusion (AGID) assay that uses BLV cultivated in Fetal Lamb Kidney cells is the only assay produced in Brazil and used in most laboratories for EBL diagnosis. Aiming to fulfil this gap, we developed an indirect ELISA based on the recombinant capsid protein (p24) of BLV to detect antibodies in cattle. To reach our goals, we designed PCR primers to amplify the nucleotides coding for the p24 protein and cloned the resulting DNA fragment in the pET-20 plasmid. The resulting plasmid was transformed in competent E. coli ER2566 and the protein expression was induced by IPTG (0.1mM). The protein (BLVp24r) was purified using a HisTrap column coupled to an ÄKTA Pure Chromatography equipment, and later analyzed by SDS-PAGE. The antigenicity and immunogenicity of the BLVp24r were evaluated by Western blot using sera from rats immunized with BLVrp24 and with sera from naturally infected cows prior to the development of the ELISA. For the ELISA, the microplate type, antigen concentration and serum dilution were determined by checkboard analysis. The receptor operation characteristics (ROC) curve analysis and the area under the curve (AUC) analysis were used to evaluate the ELISA performance. After that, the ELISA was used to evaluate the prevalence of anti-BLV antibodies in cattle blood. The BLVp24r protein was expressed as a fusion protein and had a molecular mass of 67 KDa. Only the serum from immunized rats and from cattle naturally infected with BLV recognized the BLVp24r by Western blot. The PolySorp® plates provide the bestperformance on the BLVp24r ELISA with 50 ng/well of the protein and with bovine serum diluted 1:100. Our indirect ELISA to BLV was set with a cut-off value of 0.320 at OD450nm and had sensibility of 98.5% and 100% specificity. The ROC had an AUC value of 0.9989 (95% confidence interval from 0.9961 to 1.002), indicating high level of precision. With this ELISA we screened sera samples from cattle and found a prevalence of antibodies to BLV in 31.1% of dairy cattle and 9.5% in beef cattle. The BLVp24r is suitable to detect antibodies to BLV in bovine serum by ELISA and should be a strong candidate for the development of a commercial assay aimingto control EBL in cattle.O vírus da leucemia bovina (BLV) é o agente etiológico da leucose enzoótica bovina (LEB), uma doença infecciosa persistente e altamente prevalente no gado leiteiro. Testes sorológicos e remoção de animais infectados são fundamentais para o controle da doença. No Brasil, a imunodifusão em gel de ágar (IDGA) usando o BLV produzido em cultivo de células de rim fetal de carneiro é o único teste comercial genuinamente brasileiro disponível para o diagnóstico da LEB. Para suprir essa deficiência no diagnóstico, desenvolvemos um ELISA indireto com base na proteína recombinante do capsídeo viral (p24) do BLV para detectar anticorpos em bovinos com diferentes aptidões. Para isso, foi desenhado um par de primer para amplificar por meio da PCR a sequência de nucleotídeos que codifica a proteína p24, clonando o DNA resultante no plasmídeo pET-20. O plasmídeo foi clonado em Escherichia coli ER2566 cálcio-competente e a expressão da proteína foi induzida com IPTG (0.1mM). A proteína resultante (BLVp24r) foi purificada pelo sistema de cromatografia através da coluna HisTrap acoplada no equipamento ÄKTA Pure Chromatography e, posteriormente, analisada por SDS-PAGE. As características de antigenicidade e imunogenicidade da BLVp24r foram avaliadas através da técnica de Western Blot, utilizando soro policlonal de ratos imunizados com a BLVp24r e soro de bovinos naturalmente infectados, para posterior desenvolvimento do ELISA. Para o ELISA, o tipo de microplaca, a concentração de antígeno e a diluição de soro ideal foram determinados por titulação seriada das amostras. A análise da curva de Característica de Operação do Receptor (ROC) e a Análise de Área sob Curva (AUC) foram utilizadas para avaliar o desempenho do ELISA desenvolvido. Ao fim da padronização, realizamos um estudo soroepidemiológico da prevalência de anticorpos anti-BLV em soros de bovinos. A proteína BLVp24r foi expressa com a proteína de fusão com peso molecular de 67 KDa.. O soro de ratos imunizados e soro de bovinos naturalmente infectados com BLV reconheceram somente a proteína BLVp24r por Western Blot. A microplaca Polysorp® obteve melhor performance no ELISA com BLVp24r utilizando 50 ng/poço de proteína e soro bovino diluído a 1:100. O ELISA indireto padronizado para BLV possui um cut-off de 0.320 na OD450nm e apresentando uma sensibilidade de 98.5% e especificidade de 100%. A ROC representa um valor da ASC de 0,9989 (intervalo de confiança de 95% de 0,9961 em 1,002; p <0,0001), o que indica um alto nível de precisão. Com o ELISA padronizado, realizamos um estudo soroepidemiológico para validação do teste utilizando soros bovinos, demonstrando que a prevalência de anticorpos para o BLV foi de 31.1% em bovinos de leite e de 9.5% em bovinos de corte. O ELISA desenvolvido e otimizado utilizando a BLVp24r como antígeno é adequado para detectar anticorpos anti-BLV em soros bovinos e pode ser considerado um forte candidato a kit comercial visando o controle de BLV em bovinos.Submitted by Mariana Freitas (marianafreitas@upf.br) on 2018-12-18T19:24:52Z No. of bitstreams: 1 2017AnaPaulaAndreolla.pdf: 832595 bytes, checksum: 96201146a971a14939642d1312de0e37 (MD5)Made available in DSpace on 2018-12-18T19:24:52Z (GMT). No. of bitstreams: 1 2017AnaPaulaAndreolla.pdf: 832595 bytes, checksum: 96201146a971a14939642d1312de0e37 (MD5) Previous issue date: 2017-08-07application/pdfporUniversidade de Passo FundoPrograma de Pós-Graduação em BioexperimentaçãoUPFBrasilFaculdade de Agronomia e Medicina Veterinária – FAMVBovinoTeste imunoenzimáticoDiagnósticoCIENCIAS AGRARIAS::MEDICINA VETERINARIADesenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinosDevelopment of an indirect in-house ELISA based on recombinant p24 protein for the diagnosis of enzootic leukosis in cattleinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesis79452006251700495950050060053202200503672799453670264235017319info:eu-repo/semantics/openAccessreponame:Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF)instname:Universidade de Passo Fundo (UPF)instacron:UPFLICENSElicense.txtlicense.txttext/plain; charset=utf-81940http://tede.upf.br:8080/jspui/bitstream/tede/1590/1/license.txte0faded76e3df80302a4a0fb3f2bb5f3MD51ORIGINAL2017AnaPaulaAndreolla.pdf2017AnaPaulaAndreolla.pdfapplication/pdf832595http://tede.upf.br:8080/jspui/bitstream/tede/1590/2/2017AnaPaulaAndreolla.pdf96201146a971a14939642d1312de0e37MD52tede/15902018-12-18 17:24:52.17oai:tede.upf.br: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Biblioteca Digital de Teses e DissertaçõesPUBhttp://tede.upf.br/oai/requestbiblio@upf.br \|\| bio@upf.br \|\| cas@upf.br \|\| car@upf.br \|\| lve@upf.br \|\| sar@upf.br \|\| sol@upf.br \|\| upfmundi@upf.br \|\| jucelei@upf.bropendoar:2018-12-18T19:24:52Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF) - Universidade de Passo Fundo (UPF)false
dc.title.por.fl_str_mv	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
dc.title.alternative.eng.fl_str_mv	Development of an indirect in-house ELISA based on recombinant p24 protein for the diagnosis of enzootic leukosis in cattle
title	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
spellingShingle	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos Andreolla, Ana Paula Bovino Teste imunoenzimático Diagnóstico CIENCIAS AGRARIAS::MEDICINA VETERINARIA
title_short	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
title_full	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
title_fullStr	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
title_full_unstemmed	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
title_sort	Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos
author	Andreolla, Ana Paula
author_facet	Andreolla, Ana Paula
author_role	author
dc.contributor.advisor1.fl_str_mv	Kreutz, Luiz Carlos
dc.contributor.advisor1ID.fl_str_mv	56057555953
dc.contributor.advisor1Lattes.fl_str_mv	http://lattes.cnpq.br/6207090944092820
dc.contributor.authorID.fl_str_mv	01947247000
dc.contributor.authorLattes.fl_str_mv	http://lattes.cnpq.br/5525234743711148
dc.contributor.author.fl_str_mv	Andreolla, Ana Paula
contributor_str_mv	Kreutz, Luiz Carlos
dc.subject.por.fl_str_mv	Bovino Teste imunoenzimático Diagnóstico
topic	Bovino Teste imunoenzimático Diagnóstico CIENCIAS AGRARIAS::MEDICINA VETERINARIA
dc.subject.cnpq.fl_str_mv	CIENCIAS AGRARIAS::MEDICINA VETERINARIA
description	Bovine Leukemia Virus (BLV) is the etiological agent of enzootic bovine leukemia (EBL) a persistent infectious disease highly prevalent in dairy cattle. Serological testing and culling infected animals are central to disease control. The agar gel immunodiffusion (AGID) assay that uses BLV cultivated in Fetal Lamb Kidney cells is the only assay produced in Brazil and used in most laboratories for EBL diagnosis. Aiming to fulfil this gap, we developed an indirect ELISA based on the recombinant capsid protein (p24) of BLV to detect antibodies in cattle. To reach our goals, we designed PCR primers to amplify the nucleotides coding for the p24 protein and cloned the resulting DNA fragment in the pET-20 plasmid. The resulting plasmid was transformed in competent E. coli ER2566 and the protein expression was induced by IPTG (0.1mM). The protein (BLVp24r) was purified using a HisTrap column coupled to an ÄKTA Pure Chromatography equipment, and later analyzed by SDS-PAGE. The antigenicity and immunogenicity of the BLVp24r were evaluated by Western blot using sera from rats immunized with BLVrp24 and with sera from naturally infected cows prior to the development of the ELISA. For the ELISA, the microplate type, antigen concentration and serum dilution were determined by checkboard analysis. The receptor operation characteristics (ROC) curve analysis and the area under the curve (AUC) analysis were used to evaluate the ELISA performance. After that, the ELISA was used to evaluate the prevalence of anti-BLV antibodies in cattle blood. The BLVp24r protein was expressed as a fusion protein and had a molecular mass of 67 KDa. Only the serum from immunized rats and from cattle naturally infected with BLV recognized the BLVp24r by Western blot. The PolySorp® plates provide the bestperformance on the BLVp24r ELISA with 50 ng/well of the protein and with bovine serum diluted 1:100. Our indirect ELISA to BLV was set with a cut-off value of 0.320 at OD450nm and had sensibility of 98.5% and 100% specificity. The ROC had an AUC value of 0.9989 (95% confidence interval from 0.9961 to 1.002), indicating high level of precision. With this ELISA we screened sera samples from cattle and found a prevalence of antibodies to BLV in 31.1% of dairy cattle and 9.5% in beef cattle. The BLVp24r is suitable to detect antibodies to BLV in bovine serum by ELISA and should be a strong candidate for the development of a commercial assay aimingto control EBL in cattle.
publishDate	2017
dc.date.issued.fl_str_mv	2017-08-07
dc.date.accessioned.fl_str_mv	2018-12-18T19:24:52Z
dc.type.status.fl_str_mv	info:eu-repo/semantics/publishedVersion
dc.type.driver.fl_str_mv	info:eu-repo/semantics/masterThesis
format	masterThesis
status_str	publishedVersion
dc.identifier.citation.fl_str_mv	ANDREOLLA, Ana Paula. Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos. 2017. 49 f. Dissertação (Mestrado em Bioexperimentação) - Universidade de Passo Fundo, Passo Fundo, RS, 2017.
dc.identifier.uri.fl_str_mv	http://tede.upf.br/jspui/handle/tede/1590
identifier_str_mv	ANDREOLLA, Ana Paula. Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos. 2017. 49 f. Dissertação (Mestrado em Bioexperimentação) - Universidade de Passo Fundo, Passo Fundo, RS, 2017.
url	http://tede.upf.br/jspui/handle/tede/1590
dc.language.iso.fl_str_mv	por
language	por
dc.relation.program.fl_str_mv	794520062517004959
dc.relation.confidence.fl_str_mv	500 500 600
dc.relation.department.fl_str_mv	53202200503672799
dc.relation.cnpq.fl_str_mv	453670264235017319
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	Universidade de Passo Fundo
dc.publisher.program.fl_str_mv	Programa de Pós-Graduação em Bioexperimentação
dc.publisher.initials.fl_str_mv	UPF
dc.publisher.country.fl_str_mv	Brasil
dc.publisher.department.fl_str_mv	Faculdade de Agronomia e Medicina Veterinária – FAMV
publisher.none.fl_str_mv	Universidade de Passo Fundo
dc.source.none.fl_str_mv	reponame:Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF) instname:Universidade de Passo Fundo (UPF) instacron:UPF
instname_str	Universidade de Passo Fundo (UPF)
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reponame_str	Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF)
collection	Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF)
bitstream.url.fl_str_mv	http://tede.upf.br:8080/jspui/bitstream/tede/1590/1/license.txt http://tede.upf.br:8080/jspui/bitstream/tede/1590/2/2017AnaPaulaAndreolla.pdf
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repository.mail.fl_str_mv	biblio@upf.br \|\| bio@upf.br \|\| cas@upf.br \|\| car@upf.br \|\| lve@upf.br \|\| sar@upf.br \|\| sol@upf.br \|\| upfmundi@upf.br \|\| jucelei@upf.br
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Desenvolvimento de um ELISA in house indireto baseado na proteína p24 recombinante para diagnóstico da leucose enzoótica em bovinos

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