Purificação e identificação de proteína de Babesia bovis com atividade lectínica

Detalhes bibliográficos
Autor(a) principal: Santos, Eliziária Cardoso dos
Data de Publicação: 2011
Tipo de documento: Dissertação
Idioma: por
Título da fonte: LOCUS Repositório Institucional da UFV
Texto Completo: http://locus.ufv.br/handle/123456789/2333
Resumo: The present study aimed to purify and identify merozoite protein of B. bovis with lectin activity. For such, total soluble merozoite antigens (Bb-STAg) were subjected to affinity chromatography on immobilized fetuin agarose column. The resin adsorbed protein, eluted with NaCl, was named Fetuin Binding Protein (FBP-B.bovis). The homogeneity and characterization of molecular weight of FBP were assessed by SDS-PAGE, that revealed the protein band of 27 kilodaltons which wasn t glycosylated when combined with Pro-Q Emerald 300 glycoprotein Stain. To identify the constituent of the sample, the protein spot was cut from the gel, chemically treated and had their internal amino acids sequenced by mass spectrometry. The sequence analysis showed that the fragment was related to the bovine serum albumin of Bos taurus with mass/charge of 1567.726 in the most intense peak with score of 62 and 98,98% confidence. The fraction of the FBP-B. bovis was also subjected to sequencing of the NH2-terminal region by Automatic Edman degradation analysis which analysis in the BLAST, involving all the microorganisms, identified the following as part of a putative protein uncharacterized of Dappu pulex (flea d 'water), with E-value of 6.5, 90% identity, 90% of positivity and mass about 26.939 kilodaltons. Considering the same sequence, other BLAST analysis restricted to organisms of Apicomplexa phylum was made, and their amino acid sequence was identify as putative protein of B. bovis evolutionarily conserved with total score of 52,8, covering 71% and E-value 0.40. The isolated protein fragment was also used to immunize BALB/c mice to produce of specific antibodies that after being purified by affinity chromatography were titrated by Dot-ELISA that results in recognition of FBP-B. bovis (title 102,400). That away, was possible to obtain a protein fraction of merozoite of B. bovis with lectin activity, with the internal amino acid belonging to the protein bovine albumin serum and amino acids of the NH2-terminal region belonging to a putative protein of B. bovis that was recognized by specific anti-FBP B. bovis. According to the results presented, we believe this protein fraction of merozoite of B. bovis with lectin activity purified can be one important mediators involved in erythrocyte parasitemia. In future studies, it is proven hypothesis, it may open perspectives for new processes for therapeutic intervention against bovine babesioses and greater control of the disease.
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spelling Santos, Eliziária Cardoso doshttp://lattes.cnpq.br/4957986950044158Salcedo, Joaquín Hernán Patarroyohttp://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4783313T4Paula, Sérgio Oliveira dehttp://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4767540P4Oliveira, Leandro Licursi dehttp://lattes.cnpq.br/0578231392218162Silva, Eduardo de Almeida Marques dahttp://lattes.cnpq.br/9196320705613169Honda, Eduardo Rezendehttp://lattes.cnpq.br/58046234538581152015-03-26T13:04:13Z2012-04-232015-03-26T13:04:13Z2011-07-25SANTOS, Eliziária Cardoso dos. Purification and identification protein of Babesia bovis with lectin activity. 2011. 63 f. Dissertação (Mestrado em Análises quantitativas e moleculares do Genoma; Biologia das células e dos tecidos) - Universidade Federal de Viçosa, Viçosa, 2011.http://locus.ufv.br/handle/123456789/2333The present study aimed to purify and identify merozoite protein of B. bovis with lectin activity. For such, total soluble merozoite antigens (Bb-STAg) were subjected to affinity chromatography on immobilized fetuin agarose column. The resin adsorbed protein, eluted with NaCl, was named Fetuin Binding Protein (FBP-B.bovis). The homogeneity and characterization of molecular weight of FBP were assessed by SDS-PAGE, that revealed the protein band of 27 kilodaltons which wasn t glycosylated when combined with Pro-Q Emerald 300 glycoprotein Stain. To identify the constituent of the sample, the protein spot was cut from the gel, chemically treated and had their internal amino acids sequenced by mass spectrometry. The sequence analysis showed that the fragment was related to the bovine serum albumin of Bos taurus with mass/charge of 1567.726 in the most intense peak with score of 62 and 98,98% confidence. The fraction of the FBP-B. bovis was also subjected to sequencing of the NH2-terminal region by Automatic Edman degradation analysis which analysis in the BLAST, involving all the microorganisms, identified the following as part of a putative protein uncharacterized of Dappu pulex (flea d 'water), with E-value of 6.5, 90% identity, 90% of positivity and mass about 26.939 kilodaltons. Considering the same sequence, other BLAST analysis restricted to organisms of Apicomplexa phylum was made, and their amino acid sequence was identify as putative protein of B. bovis evolutionarily conserved with total score of 52,8, covering 71% and E-value 0.40. The isolated protein fragment was also used to immunize BALB/c mice to produce of specific antibodies that after being purified by affinity chromatography were titrated by Dot-ELISA that results in recognition of FBP-B. bovis (title 102,400). That away, was possible to obtain a protein fraction of merozoite of B. bovis with lectin activity, with the internal amino acid belonging to the protein bovine albumin serum and amino acids of the NH2-terminal region belonging to a putative protein of B. bovis that was recognized by specific anti-FBP B. bovis. According to the results presented, we believe this protein fraction of merozoite of B. bovis with lectin activity purified can be one important mediators involved in erythrocyte parasitemia. In future studies, it is proven hypothesis, it may open perspectives for new processes for therapeutic intervention against bovine babesioses and greater control of the disease.O presente estudo objetivou purificar e identificar uma proteína de merozoíto de B. bovis com atividade lectínica. Para tal, antígenos solúveis totais de merozoíto foram submetidos à cromatografia de afinidade em coluna de agarose fetuína imobilizada. A fração protéica adsorvida à resina e eluída com cloreto de sódio foi denominada Fetuin Binding Protein (FBP) B. bovis. A homogeneidade e a caracterização da FBP quanto à massa molecular foram avaliados por SDS-PAGE, que revelou uma banda protéica na altura de 27 kDa, a qual não apresentou glicosilações quando conjugada com Pro-Q Emerald 300 glycoprotein Stain. Para identificar a constituição da amostra, à banda correspondente à fração protéica foi recortado do gel, tratada quimicamente e teve seus aminoácidos internos sequenciados por Espectrometria de Massa. A análise da sequência evidenciou que o fragmento era referente à albumina sérica bovina de Bos taurus com relação massa carga (m/z) de 1567,726 no pico mais intenso e com um score de 62 e 98, 98% de confiabilidade. Uma fração da FBP-B. bovis foi ainda submetida a sequenciamento da região NH2-terminal por Degradação Automática de Edman, cuja análise no algoritmo BLAST, envolvendo todos os microorganismos, identificou a sequência como sendo parte de uma proteína putativa não caracterizada de Dappu pulex (pulga d água), com um E-value de 6,5, 90% de identidade, 90% de positividade e massa aproximada de 26,939 Kilodaltons. Considerando a mesma sequência, outra análise no BLAST, restrita aos organismos do filo apicomplexa, foi realizada tendo seus aminoácidos identificados dentro da sequência de uma proteína putativa de B. bovis conservada evolutivamente com um score total de 52,8, cobertura de 71% e E-value de 0,40. O fragmento protéico isolado foi ainda utilizado para imunizar camundongos BALB/c para a produção de anticorpos específicos que, após serem purificados por cromatografia de afinidade, foram titulados por Dot-Elisa e reconheceram a FBP-B. bovis até o título de 102.400. Desta forma, foi obtida uma proteína de merozoíto de B. bovis com atividade lectínica, com os aminoácidos internos pertencentes à proteína albumina sérica bovina e os aminoácidos da região NH2-terminal a uma proteína putativa de B. bovis que foi reconhecida por anticorpos específicos anti-FBP B. bovis. De acordo com os resultados apresentados, acredita-se que a proteína com atividade lectínica de merozoíto de B. bovis purificada possa ser um dos mediadores envolvidos na parasitemia dos eritrócitos. Em estudos futuros, se comprovada esta hipótese, ela pode abrir perspectivas para novos processos de intervenção terapêutica contra a Babesiose bovina e maior controle da doença.Coordenação de Aperfeiçoamento de Pessoal de Nível Superiorapplication/pdfporUniversidade Federal de ViçosaMestrado em Biologia Celular e EstruturalUFVBRAnálises quantitativas e moleculares do Genoma; Biologia das células e dos tecidosBabesiaLectinaBabesiaLectinCNPQ::CIENCIAS BIOLOGICAS::BIOLOGIA GERALPurificação e identificação de proteína de Babesia bovis com atividade lectínicaPurification and identification protein of Babesia bovis with lectin activityinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesisinfo:eu-repo/semantics/openAccessreponame:LOCUS Repositório Institucional da UFVinstname:Universidade Federal de Viçosa (UFV)instacron:UFVORIGINALtexto completo.pdfapplication/pdf1187986https://locus.ufv.br//bitstream/123456789/2333/1/texto%20completo.pdfb9f348b3b08194a6ce376bd651e005edMD51TEXTtexto completo.pdf.txttexto completo.pdf.txtExtracted texttext/plain103721https://locus.ufv.br//bitstream/123456789/2333/2/texto%20completo.pdf.txt2822b0296e0d18356aa23dee73ddc2b7MD52THUMBNAILtexto completo.pdf.jpgtexto completo.pdf.jpgIM Thumbnailimage/jpeg3645https://locus.ufv.br//bitstream/123456789/2333/3/texto%20completo.pdf.jpg7b5550263e9a17bee0c890c09075c4f8MD53123456789/23332016-04-08 23:05:21.79oai:locus.ufv.br:123456789/2333Repositório InstitucionalPUBhttps://www.locus.ufv.br/oai/requestfabiojreis@ufv.bropendoar:21452016-04-09T02:05:21LOCUS Repositório Institucional da UFV - Universidade Federal de Viçosa (UFV)false
dc.title.por.fl_str_mv Purificação e identificação de proteína de Babesia bovis com atividade lectínica
dc.title.alternative.eng.fl_str_mv Purification and identification protein of Babesia bovis with lectin activity
title Purificação e identificação de proteína de Babesia bovis com atividade lectínica
spellingShingle Purificação e identificação de proteína de Babesia bovis com atividade lectínica
Santos, Eliziária Cardoso dos
Babesia
Lectina
Babesia
Lectin
CNPQ::CIENCIAS BIOLOGICAS::BIOLOGIA GERAL
title_short Purificação e identificação de proteína de Babesia bovis com atividade lectínica
title_full Purificação e identificação de proteína de Babesia bovis com atividade lectínica
title_fullStr Purificação e identificação de proteína de Babesia bovis com atividade lectínica
title_full_unstemmed Purificação e identificação de proteína de Babesia bovis com atividade lectínica
title_sort Purificação e identificação de proteína de Babesia bovis com atividade lectínica
author Santos, Eliziária Cardoso dos
author_facet Santos, Eliziária Cardoso dos
author_role author
dc.contributor.authorLattes.por.fl_str_mv http://lattes.cnpq.br/4957986950044158
dc.contributor.author.fl_str_mv Santos, Eliziária Cardoso dos
dc.contributor.advisor-co1.fl_str_mv Salcedo, Joaquín Hernán Patarroyo
dc.contributor.advisor-co1Lattes.fl_str_mv http://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4783313T4
dc.contributor.advisor-co2.fl_str_mv Paula, Sérgio Oliveira de
dc.contributor.advisor-co2Lattes.fl_str_mv http://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4767540P4
dc.contributor.advisor1.fl_str_mv Oliveira, Leandro Licursi de
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/0578231392218162
dc.contributor.referee1.fl_str_mv Silva, Eduardo de Almeida Marques da
dc.contributor.referee1Lattes.fl_str_mv http://lattes.cnpq.br/9196320705613169
dc.contributor.referee2.fl_str_mv Honda, Eduardo Rezende
dc.contributor.referee2Lattes.fl_str_mv http://lattes.cnpq.br/5804623453858115
contributor_str_mv Salcedo, Joaquín Hernán Patarroyo
Paula, Sérgio Oliveira de
Oliveira, Leandro Licursi de
Silva, Eduardo de Almeida Marques da
Honda, Eduardo Rezende
dc.subject.por.fl_str_mv Babesia
Lectina
topic Babesia
Lectina
Babesia
Lectin
CNPQ::CIENCIAS BIOLOGICAS::BIOLOGIA GERAL
dc.subject.eng.fl_str_mv Babesia
Lectin
dc.subject.cnpq.fl_str_mv CNPQ::CIENCIAS BIOLOGICAS::BIOLOGIA GERAL
description The present study aimed to purify and identify merozoite protein of B. bovis with lectin activity. For such, total soluble merozoite antigens (Bb-STAg) were subjected to affinity chromatography on immobilized fetuin agarose column. The resin adsorbed protein, eluted with NaCl, was named Fetuin Binding Protein (FBP-B.bovis). The homogeneity and characterization of molecular weight of FBP were assessed by SDS-PAGE, that revealed the protein band of 27 kilodaltons which wasn t glycosylated when combined with Pro-Q Emerald 300 glycoprotein Stain. To identify the constituent of the sample, the protein spot was cut from the gel, chemically treated and had their internal amino acids sequenced by mass spectrometry. The sequence analysis showed that the fragment was related to the bovine serum albumin of Bos taurus with mass/charge of 1567.726 in the most intense peak with score of 62 and 98,98% confidence. The fraction of the FBP-B. bovis was also subjected to sequencing of the NH2-terminal region by Automatic Edman degradation analysis which analysis in the BLAST, involving all the microorganisms, identified the following as part of a putative protein uncharacterized of Dappu pulex (flea d 'water), with E-value of 6.5, 90% identity, 90% of positivity and mass about 26.939 kilodaltons. Considering the same sequence, other BLAST analysis restricted to organisms of Apicomplexa phylum was made, and their amino acid sequence was identify as putative protein of B. bovis evolutionarily conserved with total score of 52,8, covering 71% and E-value 0.40. The isolated protein fragment was also used to immunize BALB/c mice to produce of specific antibodies that after being purified by affinity chromatography were titrated by Dot-ELISA that results in recognition of FBP-B. bovis (title 102,400). That away, was possible to obtain a protein fraction of merozoite of B. bovis with lectin activity, with the internal amino acid belonging to the protein bovine albumin serum and amino acids of the NH2-terminal region belonging to a putative protein of B. bovis that was recognized by specific anti-FBP B. bovis. According to the results presented, we believe this protein fraction of merozoite of B. bovis with lectin activity purified can be one important mediators involved in erythrocyte parasitemia. In future studies, it is proven hypothesis, it may open perspectives for new processes for therapeutic intervention against bovine babesioses and greater control of the disease.
publishDate 2011
dc.date.issued.fl_str_mv 2011-07-25
dc.date.available.fl_str_mv 2012-04-23
2015-03-26T13:04:13Z
dc.date.accessioned.fl_str_mv 2015-03-26T13:04:13Z
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dc.type.driver.fl_str_mv info:eu-repo/semantics/masterThesis
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dc.identifier.citation.fl_str_mv SANTOS, Eliziária Cardoso dos. Purification and identification protein of Babesia bovis with lectin activity. 2011. 63 f. Dissertação (Mestrado em Análises quantitativas e moleculares do Genoma; Biologia das células e dos tecidos) - Universidade Federal de Viçosa, Viçosa, 2011.
dc.identifier.uri.fl_str_mv http://locus.ufv.br/handle/123456789/2333
identifier_str_mv SANTOS, Eliziária Cardoso dos. Purification and identification protein of Babesia bovis with lectin activity. 2011. 63 f. Dissertação (Mestrado em Análises quantitativas e moleculares do Genoma; Biologia das células e dos tecidos) - Universidade Federal de Viçosa, Viçosa, 2011.
url http://locus.ufv.br/handle/123456789/2333
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dc.publisher.program.fl_str_mv Mestrado em Biologia Celular e Estrutural
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dc.publisher.country.fl_str_mv BR
dc.publisher.department.fl_str_mv Análises quantitativas e moleculares do Genoma; Biologia das células e dos tecidos
publisher.none.fl_str_mv Universidade Federal de Viçosa
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