Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis

Detalhes bibliográficos
Autor(a) principal: Barasuol, Bibiana Martins
Data de Publicação: 2016
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/1601
Resumo: In this study, through in vitro assays, we present the functional characterization the antibody against transferrin binding protein B (TbpB) from Haemophilus parasuis. Four recombinant antigen-based on the protein structure of TbpB were developed and evaluated in this study. The intact TbpB protein (TbpB-I20-528aa, mutant TbpB TbpB-M26-528aa and subdomains (lobes) NTbpB-Nm 20-282aa mutant version) and C TbpB-C283-528aa of TbpB from H. parasuis, serotype 5, Nagasaki strain, were cloned into pET20 expression vector and expressed in cells of Escherichia coli, strain ER 2566. The recombinant antigens were purified by liquid chromatography. Pigs were immunized with recombinant antigens adjuvanted with the adjuvant Montanide IMS 2215 VG PR and, the kinetics of antibody response was assessed by indirect ELISA. The antisera capacity to recognize 6 virulent strains of H. parasuis (Nº4 – Serovar (SV) 1, SW124 – SV4, Nagasaki – SV5, H425 – SV12, 84-22113 – SV14 e 84-15995 – SV15) was analyzed by flow cytometry, as well as the effect of antibodies opsonization during the H. parasuis phagocytosis performed by swine neutrophils. Finally, we analyze the ability of different antisera to activate the classical pathway of the complement system and to produce the killing of bacteria through antibody-mediated bactericidal assay. The results presented in this study demonstrate that all recombinant antigens were immunogenic in pigs and, that higher titres of antibodies were induced by antigens TbpB-M and TbpB-C, respectively. Except for SV4, all others serovars (SV1, SV5, SV12, SV14 e SV15) were strongly recognized (60-90%) by one or more specific antisera, demonstrating that TbpB protein from 6 virulent serovars analyzed share conserved epitopes in both lobes, N and C of the TbpB protein. In general, the number of antibodies associated with the strains was lower when we used the antisera produced with TbpB-I antigen. Interestingly, we observed that the homogenous expression of native TbpB protein from H. parasuis (independently of serovar) is only achieved if the microorganism is growth in iron starvation. Regarding the phagocytosis, we observed that the opsonization process, independently of the specific type of antibody, have increased the number of neutrophils with associated bacteria, as well, the number of bacteria captured by each neutrophil. The percentage of neutrophils with internalized bacteria was significantly higher when the microorganism was opsonized, however, this process seems to be slower against the SV12. Surprisingly, none of the swine antisera was capable of activating the classical pathway of the complement system (CPCS), suggesting that the Montanide IMS 2215 VG adjuvant has induced an antibody isotype with reduced functional activity in pigs. On the other hand, antibodies produced in mice against the TbpB-M, TbpB-Nm and TbpB-C protein adjuvanted with Freund adjuvant and/or Montanide Gel 01 were able to activate CPCS against all sevorars included. In summary, we demonstrate in this study, the functional activity of specific antibodies generated against four recombinant antigens based on the structure of TbpB protein from H. parasuis. The results presented are useful to predict in vitro the capacity of homologous and heterologous protection of vaccines based on these antigens.
id UPF-1_6e9da6ba3fa50e4454d3870ea7dd1b8b
oai_identifier_str oai:tede.upf.br:tede/1601
network_acronym_str UPF-1
network_name_str Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF)
repository_id_str
spelling Frandoloso, Rafael03912065918http://lattes.cnpq.br/250289135401741001858646006http://lattes.cnpq.br/7844951925880855Barasuol, Bibiana Martins2019-01-03T12:34:13Z2016-08-19BARASUOL, Bibiana Martins. Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis. 2016. 68 f. Dissertação (Mestrado em Bioexperimentação) - Universidade de Passo Fundo, Passo Fundo, RS, 2016.http://tede.upf.br/jspui/handle/tede/1601In this study, through in vitro assays, we present the functional characterization the antibody against transferrin binding protein B (TbpB) from Haemophilus parasuis. Four recombinant antigen-based on the protein structure of TbpB were developed and evaluated in this study. The intact TbpB protein (TbpB-I20-528aa, mutant TbpB TbpB-M26-528aa and subdomains (lobes) NTbpB-Nm 20-282aa mutant version) and C TbpB-C283-528aa of TbpB from H. parasuis, serotype 5, Nagasaki strain, were cloned into pET20 expression vector and expressed in cells of Escherichia coli, strain ER 2566. The recombinant antigens were purified by liquid chromatography. Pigs were immunized with recombinant antigens adjuvanted with the adjuvant Montanide IMS 2215 VG PR and, the kinetics of antibody response was assessed by indirect ELISA. The antisera capacity to recognize 6 virulent strains of H. parasuis (Nº4 – Serovar (SV) 1, SW124 – SV4, Nagasaki – SV5, H425 – SV12, 84-22113 – SV14 e 84-15995 – SV15) was analyzed by flow cytometry, as well as the effect of antibodies opsonization during the H. parasuis phagocytosis performed by swine neutrophils. Finally, we analyze the ability of different antisera to activate the classical pathway of the complement system and to produce the killing of bacteria through antibody-mediated bactericidal assay. The results presented in this study demonstrate that all recombinant antigens were immunogenic in pigs and, that higher titres of antibodies were induced by antigens TbpB-M and TbpB-C, respectively. Except for SV4, all others serovars (SV1, SV5, SV12, SV14 e SV15) were strongly recognized (60-90%) by one or more specific antisera, demonstrating that TbpB protein from 6 virulent serovars analyzed share conserved epitopes in both lobes, N and C of the TbpB protein. In general, the number of antibodies associated with the strains was lower when we used the antisera produced with TbpB-I antigen. Interestingly, we observed that the homogenous expression of native TbpB protein from H. parasuis (independently of serovar) is only achieved if the microorganism is growth in iron starvation. Regarding the phagocytosis, we observed that the opsonization process, independently of the specific type of antibody, have increased the number of neutrophils with associated bacteria, as well, the number of bacteria captured by each neutrophil. The percentage of neutrophils with internalized bacteria was significantly higher when the microorganism was opsonized, however, this process seems to be slower against the SV12. Surprisingly, none of the swine antisera was capable of activating the classical pathway of the complement system (CPCS), suggesting that the Montanide IMS 2215 VG adjuvant has induced an antibody isotype with reduced functional activity in pigs. On the other hand, antibodies produced in mice against the TbpB-M, TbpB-Nm and TbpB-C protein adjuvanted with Freund adjuvant and/or Montanide Gel 01 were able to activate CPCS against all sevorars included. In summary, we demonstrate in this study, the functional activity of specific antibodies generated against four recombinant antigens based on the structure of TbpB protein from H. parasuis. The results presented are useful to predict in vitro the capacity of homologous and heterologous protection of vaccines based on these antigens.Neste estudo, através de ensaios in vitro, apresentamos a caracterização funcional de anticorpos contra a proteína de união à transferrina B (TbpB) de Haemophilus parasuis. Quatro antígenos recombinantes baseados na estrutura da proteína TbpB foram desenvolvidos e avaliados neste estudo. As proteínas TbpB intacta (TbpB-I20-528aa), TbpB mutante [TbpB-M26-528aa (Frandoloso, et al. 2015)] e os subdomínios (lóbulos) N (TbpB-Nm20-282aa, versão mutante) e C (TbpB-C283-528aa) da TbpB de H. parasuis, sorovar 5, cepa Nagasaki, foram clonadas no vetor de expressão pET20 e expressadas em células de Escherichia coli cepa ER2566. A purificação dos antígenos foi realizada mediante cromatografia líquida de proteína. Suínos foram imunizados com os antígenos recombinantes potencializados com o adjuvante Montanide IMS 2215 VG PR e, a cinética da resposta de anticorpos foi analisada através de um ELISA indireto. A capacidade dos antissoros de reconhecerem 5 cepas virulentas de H. parasuis (Nº4 ¿ Sorovar (SV) 1; SW124 ¿ SV4; Nagasaki ¿ SV5; H425 ¿ SV12; 84-22113 ¿ SV14 e 84-15995 ¿ SV15) foi avaliada por citometria de fluxo, como também o efeito opsonizante dos anticorpos durante a fagocitose de H. parasuis realizada por neutrófilos suínos. Por último, analisou-se a capacidade dos diferentes antissoros de fixar a via clássica do sistema do complemento e, de produzir a morte das bactérias através de um ensaio bactericida mediado por anticorpos. Os resultados apresentados neste estudo demonstram que todos os antígenos recombinantes foram imunogênicos em suínos e, que os títulos de anticorpos mais elevados foram induzidos pelos antígenos TbpB-M e TbpB-C. Com exceção do SV4, todos os demais sorovares (SV1, SV5, SV12, SV14 e SV15) foram altamente reconhecidos (60 ¿ 90%) por um ou mais antissoros específicos, demonstrando que a proteína TbpB dos 5 sorovares virulentos analisados compartilham epítopos conservados tanto no lóbulo N e no lóbulo C da proteína TbpB. De maneira geral, o número de anticorpos associados às cepas avaliadas foi menor quando utilizou-se os antissoros produzidos com o antígeno TbpB-I. Interessantemente, observamos que a expressão homogênea da proteína TbpB nativa de H. parasuis (independente do sorovar) somente alcançada se o microrganismo for cultivado em condições restritivas de ferro. Com relação a fagocitose, observamos que o processo de opsonização, independente do tipo de anticorpo específico aumentou significativamente o número de neutrófilos com bactérias associadas, bem como o número de bactérias capturadas por cada neutrófilos. A porcentagem de neutrófilos com bactérias internalizadas foi significativamente maior quando os microrganismos estavam opsonizados, no entanto, este processo parece ser mais lento contra o SV12. Surpreendentemente, nenhum dos antissoros suínos foi capaz de ativar a via clássica do sistema do complemento (VCSC), sugerindo que o adjuvante Montanide IMS 2215 VG induza um isotipo de anticorpo com reduzida capacidade funcional em suínos. De maneira contrária, anticorpos produzidos em camundongos contra as proteínas TbpB-M TbpB-Nm e TbpB-C potencializadas com os adjuvantes de Freund e ou Montanide Gel 01 foram capazes de fixar VCSC contra todos os sorovares analisados. Em síntese, demonstramos neste estudo, a capacidade funcional dos anticorpos gerados contra 4 antígenos recombinantes baseados na estrutura da proteína TbpB de H. parasuis. Os resultados apresentados são úteis para predizer in vitro o potencial de proteção homólogo e heterólogo de vacinas baseadas nestes antígenos.Submitted by Mariana Freitas (marianafreitas@upf.br) on 2019-01-03T12:34:13Z No. of bitstreams: 1 2016BibianaBarasuol.pdf: 980334 bytes, checksum: d1377829da5431f9cf729386804d31dd (MD5)Made available in DSpace on 2019-01-03T12:34:13Z (GMT). No. of bitstreams: 1 2016BibianaBarasuol.pdf: 980334 bytes, checksum: d1377829da5431f9cf729386804d31dd (MD5) Previous issue date: 2016-08-19Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPESapplication/pdfporUniversidade de Passo FundoPrograma de Pós-Graduação em BioexperimentaçãoUPFBrasilFaculdade de Agronomia e Medicina Veterinária – FAMVEstudos soroepidemiológicosPatologia veterináriaSuínoDoençasCIENCIAS AGRARIAS::MEDICINA VETERINARIACaracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuisCharacterization of the functional immune response induced by recombinant antigens based on the structure of the tbpB protein of haemophilus parasuisinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesis794520062517004959500500600600532022005036727994536702642350173192075167498588264571info: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/1601/1/license.txte0faded76e3df80302a4a0fb3f2bb5f3MD51ORIGINAL2016BibianaBarasuol.pdf2016BibianaBarasuol.pdfapplication/pdf980334http://tede.upf.br:8080/jspui/bitstream/tede/1601/2/2016BibianaBarasuol.pdfd1377829da5431f9cf729386804d31ddMD52tede/16012019-01-03 10:34:13.862oai: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:2019-01-03T12:34:13Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF) - Universidade de Passo Fundo (UPF)false
dc.title.por.fl_str_mv Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
dc.title.alternative.eng.fl_str_mv Characterization of the functional immune response induced by recombinant antigens based on the structure of the tbpB protein of haemophilus parasuis
title Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
spellingShingle Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
Barasuol, Bibiana Martins
Estudos soroepidemiológicos
Patologia veterinária
Suíno
Doenças
CIENCIAS AGRARIAS::MEDICINA VETERINARIA
title_short Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
title_full Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
title_fullStr Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
title_full_unstemmed Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
title_sort Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis
author Barasuol, Bibiana Martins
author_facet Barasuol, Bibiana Martins
author_role author
dc.contributor.advisor1.fl_str_mv Frandoloso, Rafael
dc.contributor.advisor1ID.fl_str_mv 03912065918
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/2502891354017410
dc.contributor.authorID.fl_str_mv 01858646006
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/7844951925880855
dc.contributor.author.fl_str_mv Barasuol, Bibiana Martins
contributor_str_mv Frandoloso, Rafael
dc.subject.por.fl_str_mv Estudos soroepidemiológicos
Patologia veterinária
Suíno
Doenças
topic Estudos soroepidemiológicos
Patologia veterinária
Suíno
Doenças
CIENCIAS AGRARIAS::MEDICINA VETERINARIA
dc.subject.cnpq.fl_str_mv CIENCIAS AGRARIAS::MEDICINA VETERINARIA
description In this study, through in vitro assays, we present the functional characterization the antibody against transferrin binding protein B (TbpB) from Haemophilus parasuis. Four recombinant antigen-based on the protein structure of TbpB were developed and evaluated in this study. The intact TbpB protein (TbpB-I20-528aa, mutant TbpB TbpB-M26-528aa and subdomains (lobes) NTbpB-Nm 20-282aa mutant version) and C TbpB-C283-528aa of TbpB from H. parasuis, serotype 5, Nagasaki strain, were cloned into pET20 expression vector and expressed in cells of Escherichia coli, strain ER 2566. The recombinant antigens were purified by liquid chromatography. Pigs were immunized with recombinant antigens adjuvanted with the adjuvant Montanide IMS 2215 VG PR and, the kinetics of antibody response was assessed by indirect ELISA. The antisera capacity to recognize 6 virulent strains of H. parasuis (Nº4 – Serovar (SV) 1, SW124 – SV4, Nagasaki – SV5, H425 – SV12, 84-22113 – SV14 e 84-15995 – SV15) was analyzed by flow cytometry, as well as the effect of antibodies opsonization during the H. parasuis phagocytosis performed by swine neutrophils. Finally, we analyze the ability of different antisera to activate the classical pathway of the complement system and to produce the killing of bacteria through antibody-mediated bactericidal assay. The results presented in this study demonstrate that all recombinant antigens were immunogenic in pigs and, that higher titres of antibodies were induced by antigens TbpB-M and TbpB-C, respectively. Except for SV4, all others serovars (SV1, SV5, SV12, SV14 e SV15) were strongly recognized (60-90%) by one or more specific antisera, demonstrating that TbpB protein from 6 virulent serovars analyzed share conserved epitopes in both lobes, N and C of the TbpB protein. In general, the number of antibodies associated with the strains was lower when we used the antisera produced with TbpB-I antigen. Interestingly, we observed that the homogenous expression of native TbpB protein from H. parasuis (independently of serovar) is only achieved if the microorganism is growth in iron starvation. Regarding the phagocytosis, we observed that the opsonization process, independently of the specific type of antibody, have increased the number of neutrophils with associated bacteria, as well, the number of bacteria captured by each neutrophil. The percentage of neutrophils with internalized bacteria was significantly higher when the microorganism was opsonized, however, this process seems to be slower against the SV12. Surprisingly, none of the swine antisera was capable of activating the classical pathway of the complement system (CPCS), suggesting that the Montanide IMS 2215 VG adjuvant has induced an antibody isotype with reduced functional activity in pigs. On the other hand, antibodies produced in mice against the TbpB-M, TbpB-Nm and TbpB-C protein adjuvanted with Freund adjuvant and/or Montanide Gel 01 were able to activate CPCS against all sevorars included. In summary, we demonstrate in this study, the functional activity of specific antibodies generated against four recombinant antigens based on the structure of TbpB protein from H. parasuis. The results presented are useful to predict in vitro the capacity of homologous and heterologous protection of vaccines based on these antigens.
publishDate 2016
dc.date.issued.fl_str_mv 2016-08-19
dc.date.accessioned.fl_str_mv 2019-01-03T12:34:13Z
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 BARASUOL, Bibiana Martins. Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis. 2016. 68 f. Dissertação (Mestrado em Bioexperimentação) - Universidade de Passo Fundo, Passo Fundo, RS, 2016.
dc.identifier.uri.fl_str_mv http://tede.upf.br/jspui/handle/tede/1601
identifier_str_mv BARASUOL, Bibiana Martins. Caracterização da resposta imune funcional induzida por antígenos recombinantes baseados na estrutura da proteína tbpB de haemophilus parasuis. 2016. 68 f. Dissertação (Mestrado em Bioexperimentação) - Universidade de Passo Fundo, Passo Fundo, RS, 2016.
url http://tede.upf.br/jspui/handle/tede/1601
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
600
dc.relation.department.fl_str_mv 53202200503672799
dc.relation.cnpq.fl_str_mv 453670264235017319
dc.relation.sponsorship.fl_str_mv 2075167498588264571
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)
instacron_str UPF
institution UPF
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/1601/1/license.txt
http://tede.upf.br:8080/jspui/bitstream/tede/1601/2/2016BibianaBarasuol.pdf
bitstream.checksum.fl_str_mv e0faded76e3df80302a4a0fb3f2bb5f3
d1377829da5431f9cf729386804d31dd
bitstream.checksumAlgorithm.fl_str_mv MD5
MD5
repository.name.fl_str_mv Biblioteca de teses e dissertações da Universidade de Passo Fundo (BDTD UPF) - Universidade de Passo Fundo (UPF)
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
_version_ 1809092292738285568

Registros relacionados