Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase
| Ano de defesa: | 2017 |
|---|---|
| Autor(a) principal: | |
| Orientador(a): | |
| Banca de defesa: | |
| Tipo de documento: | Dissertação |
| Tipo de acesso: | Acesso aberto |
| Idioma: | por |
| Instituição de defesa: |
Universidade Tecnológica Federal do Paraná
Curitiba Brasil Programa de Pós-Graduação em Engenharia Biomédica UTFPR |
| Programa de Pós-Graduação: |
Não Informado pela instituição
|
| Departamento: |
Não Informado pela instituição
|
| País: |
Não Informado pela instituição
|
| Palavras-chave em Português: | |
| Link de acesso: | http://repositorio.utfpr.edu.br/jspui/handle/1/2729 |
Resumo: | The Molecular Biology Institute of Paraná (Instituto de Biologia Molecular do Paraná - IBMP) produces diagnostic kits for the Brazilian Unified National Health System (Sistema Único de Saúde - SUS), that consist in molecular tests, carried out by polymerase chain reaction (PCR). This reaction is performed by the enzyme Taq DNA Polymerase (Taq). The IBMP manufactures Taq from bacterial cell culture in accordance with Good Manufacturing Practices (GMP) and intends to produce it from a cell bank using cells from the same clone in order to increase the homogeneity and reproducibility of the production process. The objective of the present work is to establish a working cell bank (WCB) and to evaluate its stability for the production of the Taq enzyme, starting from a master cell bank (MCB) established in BioManguinhos. The WCB establishment consists of cultivating MCB colonies, characterizing them, evaluating performance, and electing proper cells to compose the WCT. The stability study contemplates tests to prove that cells retain the ability to produce Taq over time (i.e., cell viability, plasmid stability, growth kinetics, expression induction, plasmid DNA extraction and dosage, restriction analysis and plasmid evaluation). The decisive discretion for the selection of one of the clones to compose BCT was the result of growth kinetics. Stability was studied in 10 month-to-month evaluations. In them, cell viability was higher than 1,0 x 106 CFU/mL, showing that the cells remain capable of performing their metabolism and reproduction. Growth to the exponential phase occurred between 6 and 7 hours of culture, with a specific growth rate greater than 0.4 min-1 . The cultures with 1 mM IPTG expressed Taq DNA polymerase enzyme, revealing the qualification of the cells to the intended purpose. The plasmid stability was greater than 90%, indicating that the plasmid pBioMTaq remains stable and has good replication ability. The mean plasmid concentration was 338 ng/μL, and in all months it was greater than 100 ng/μL. In the restriction analysis the plasmids were correctly cleaved and in the plasmid evaluation there was adequate amplification of the 500 bp fragment, demonstrating that the plasmid remains intact and stable, with compatible sequences with its construction. The WCB was tested as substrate for a typical IBMP production process of Taq DNA polymerase, presenting satisfactory in all the stages in which it was evaluated. These results indicate that the established bank remained stable over 10 months and is apt to be used as a prototype for a WCB in compliance with GMP. |
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Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimeraseEstablishment and characterization of a working cell bank for the production of enzyme Taq DNA polymeraseEnzimasReação em cadeia de polimeraseCriopreservação de orgãos, tecidos, etcCélulasBiologia molecularSaúde públicaEngenharia biomédicaEnzymesPolymerase chain reactionCryopreservation of organs, tissues, etcCellsMolecular biologyPublic healthBiomedical engineeringCNPQ::ENGENHARIAS::ENGENHARIA BIOMEDICAEngenharia BiomédicaThe Molecular Biology Institute of Paraná (Instituto de Biologia Molecular do Paraná - IBMP) produces diagnostic kits for the Brazilian Unified National Health System (Sistema Único de Saúde - SUS), that consist in molecular tests, carried out by polymerase chain reaction (PCR). This reaction is performed by the enzyme Taq DNA Polymerase (Taq). The IBMP manufactures Taq from bacterial cell culture in accordance with Good Manufacturing Practices (GMP) and intends to produce it from a cell bank using cells from the same clone in order to increase the homogeneity and reproducibility of the production process. The objective of the present work is to establish a working cell bank (WCB) and to evaluate its stability for the production of the Taq enzyme, starting from a master cell bank (MCB) established in BioManguinhos. The WCB establishment consists of cultivating MCB colonies, characterizing them, evaluating performance, and electing proper cells to compose the WCT. The stability study contemplates tests to prove that cells retain the ability to produce Taq over time (i.e., cell viability, plasmid stability, growth kinetics, expression induction, plasmid DNA extraction and dosage, restriction analysis and plasmid evaluation). The decisive discretion for the selection of one of the clones to compose BCT was the result of growth kinetics. Stability was studied in 10 month-to-month evaluations. In them, cell viability was higher than 1,0 x 106 CFU/mL, showing that the cells remain capable of performing their metabolism and reproduction. Growth to the exponential phase occurred between 6 and 7 hours of culture, with a specific growth rate greater than 0.4 min-1 . The cultures with 1 mM IPTG expressed Taq DNA polymerase enzyme, revealing the qualification of the cells to the intended purpose. The plasmid stability was greater than 90%, indicating that the plasmid pBioMTaq remains stable and has good replication ability. The mean plasmid concentration was 338 ng/μL, and in all months it was greater than 100 ng/μL. In the restriction analysis the plasmids were correctly cleaved and in the plasmid evaluation there was adequate amplification of the 500 bp fragment, demonstrating that the plasmid remains intact and stable, with compatible sequences with its construction. The WCB was tested as substrate for a typical IBMP production process of Taq DNA polymerase, presenting satisfactory in all the stages in which it was evaluated. These results indicate that the established bank remained stable over 10 months and is apt to be used as a prototype for a WCB in compliance with GMP.O Instituto de Biologia Molecular do Paraná (IBMP) produz kits de diagnóstico para o Sistema Único de Saúde (SUS), que consistem em testes moleculares, realizados por reação em cadeia da polimerase (polymerase chain reaction - PCR). Essa reação ocorre pela atividade da enzima Taq DNA Polimerase (Taq). O IBMP fabrica a Taq a partir do cultivo de células bacterianas, em conformidade às Boas Práticas de Fabricação (BPF) e pretende produzi-la a partir de um banco de células provindas de um mesmo clone visando o aumento da homogeneidade e reprodutibilidade do processo produtivo. O objetivo do presente trabalho é estabelecer um banco de células de trabalho (BCT) e avaliar sua estabilidade para a produção da enzima Taq, partindo de um banco de células mestre (BCM) estabelecido em Bio-Manguinhos. O estabelecimento do BCT consiste em cultivar colônias do BCM, caracterizá-las, avaliar desempenho, e eleger células adequadas para compor o BCT. O estudo da estabilidade contempla testes para comprovar que as células retêm a capacidade de produzir a Taq ao longo do tempo (i.e., viabilidade celular, estabilidade plasmídica, cinética de crescimento, indução da expressão, extração e dosagem do DNA plasmidial, análise de restrição e avaliação plasmidial). O critério decisivo para a seleção de um dos clones para compor o BCT foi o resultado da cinética de crescimento. A estabilidade foi estudada em 10 avaliações realizadas mês a mês. Nelas, a viabilidade celular foi superior a 1,0 x 106 UFC/mL, mostrando que as células permanecem com capacidade de realizar seu metabolismo e reprodução. O crescimento até a fase exponencial se deu entre 6 e 7 horas de cultivo, com taxa específica de crescimento superior a 0,4 min-1 . Os cultivos acrescidos de 1 mM de IPTG expressaram a enzima Taq DNA Polimerase, revelando a qualificação das células para o fim proposto. A estabilidade plasmídica foi superior a 90%, indicando que o plasmídeo pBioMTaq se mantém estável e com boa capacidade de replicação. A concentração plasmidial média foi de 338 ng/μL, e em todos os meses foi maior que 100 ng/μL. Na análise de restrição os plasmídeos foram corretamente clivados e na avaliação plasmidial houve adequada amplificação do fragmento de 500 pb, demonstrando que o plasmídeo se mantém íntegro e estável, com sequências compatíveis com sua construção. O BCT foi testado como substrato para um processo fabril típico do IBMP de produção da Taq DNA polimerase, se apresentando satisfatório em todas as etapas em que foi avaliado. Esses resultados indicam que o banco estabelecido se manteve estável ao longo de 10 meses e está apto a ser utilizado como protótipo para um BCT em conformidade às BPF.Universidade Tecnológica Federal do ParanáCuritibaBrasilPrograma de Pós-Graduação em Engenharia BiomédicaUTFPRSchneider, Fábio Kurthttp://lattes.cnpq.br/1463591813823167Góes, Viviane Monteirohttp://lattes.cnpq.br/9583571313869062Schneider, Fábio KurtMorello, Luis GustavoSato, Gilson YukioFaria, Surian Guerios2017-12-12T18:15:18Z2017-12-12T18:15:18Z2017-02-23info:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesisapplication/pdfFARIA, Surian Guerios. Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase. 2017. 134 f. Dissertação (Mestrado em Engenharia Biomédica) - Universidade Tecnológica Federal do Paraná, Curitiba, 2017.http://repositorio.utfpr.edu.br/jspui/handle/1/2729porinfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UTFPR (da Universidade Tecnológica Federal do Paraná (RIUT))instname:Universidade Tecnológica Federal do Paraná (UTFPR)instacron:UTFPR2017-12-12T18:15:18Zoai:repositorio.utfpr.edu.br:1/2729Repositório InstitucionalPUBhttp://repositorio.utfpr.edu.br:8080/oai/requestriut@utfpr.edu.br || sibi@utfpr.edu.bropendoar:2017-12-12T18:15:18Repositório Institucional da UTFPR (da Universidade Tecnológica Federal do Paraná (RIUT)) - Universidade Tecnológica Federal do Paraná (UTFPR)false |
| dc.title.none.fl_str_mv |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase Establishment and characterization of a working cell bank for the production of enzyme Taq DNA polymerase |
| title |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase |
| spellingShingle |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase Faria, Surian Guerios Enzimas Reação em cadeia de polimerase Criopreservação de orgãos, tecidos, etc Células Biologia molecular Saúde pública Engenharia biomédica Enzymes Polymerase chain reaction Cryopreservation of organs, tissues, etc Cells Molecular biology Public health Biomedical engineering CNPQ::ENGENHARIAS::ENGENHARIA BIOMEDICA Engenharia Biomédica |
| title_short |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase |
| title_full |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase |
| title_fullStr |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase |
| title_full_unstemmed |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase |
| title_sort |
Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase |
| author |
Faria, Surian Guerios |
| author_facet |
Faria, Surian Guerios |
| author_role |
author |
| dc.contributor.none.fl_str_mv |
Schneider, Fábio Kurt http://lattes.cnpq.br/1463591813823167 Góes, Viviane Monteiro http://lattes.cnpq.br/9583571313869062 Schneider, Fábio Kurt Morello, Luis Gustavo Sato, Gilson Yukio |
| dc.contributor.author.fl_str_mv |
Faria, Surian Guerios |
| dc.subject.por.fl_str_mv |
Enzimas Reação em cadeia de polimerase Criopreservação de orgãos, tecidos, etc Células Biologia molecular Saúde pública Engenharia biomédica Enzymes Polymerase chain reaction Cryopreservation of organs, tissues, etc Cells Molecular biology Public health Biomedical engineering CNPQ::ENGENHARIAS::ENGENHARIA BIOMEDICA Engenharia Biomédica |
| topic |
Enzimas Reação em cadeia de polimerase Criopreservação de orgãos, tecidos, etc Células Biologia molecular Saúde pública Engenharia biomédica Enzymes Polymerase chain reaction Cryopreservation of organs, tissues, etc Cells Molecular biology Public health Biomedical engineering CNPQ::ENGENHARIAS::ENGENHARIA BIOMEDICA Engenharia Biomédica |
| description |
The Molecular Biology Institute of Paraná (Instituto de Biologia Molecular do Paraná - IBMP) produces diagnostic kits for the Brazilian Unified National Health System (Sistema Único de Saúde - SUS), that consist in molecular tests, carried out by polymerase chain reaction (PCR). This reaction is performed by the enzyme Taq DNA Polymerase (Taq). The IBMP manufactures Taq from bacterial cell culture in accordance with Good Manufacturing Practices (GMP) and intends to produce it from a cell bank using cells from the same clone in order to increase the homogeneity and reproducibility of the production process. The objective of the present work is to establish a working cell bank (WCB) and to evaluate its stability for the production of the Taq enzyme, starting from a master cell bank (MCB) established in BioManguinhos. The WCB establishment consists of cultivating MCB colonies, characterizing them, evaluating performance, and electing proper cells to compose the WCT. The stability study contemplates tests to prove that cells retain the ability to produce Taq over time (i.e., cell viability, plasmid stability, growth kinetics, expression induction, plasmid DNA extraction and dosage, restriction analysis and plasmid evaluation). The decisive discretion for the selection of one of the clones to compose BCT was the result of growth kinetics. Stability was studied in 10 month-to-month evaluations. In them, cell viability was higher than 1,0 x 106 CFU/mL, showing that the cells remain capable of performing their metabolism and reproduction. Growth to the exponential phase occurred between 6 and 7 hours of culture, with a specific growth rate greater than 0.4 min-1 . The cultures with 1 mM IPTG expressed Taq DNA polymerase enzyme, revealing the qualification of the cells to the intended purpose. The plasmid stability was greater than 90%, indicating that the plasmid pBioMTaq remains stable and has good replication ability. The mean plasmid concentration was 338 ng/μL, and in all months it was greater than 100 ng/μL. In the restriction analysis the plasmids were correctly cleaved and in the plasmid evaluation there was adequate amplification of the 500 bp fragment, demonstrating that the plasmid remains intact and stable, with compatible sequences with its construction. The WCB was tested as substrate for a typical IBMP production process of Taq DNA polymerase, presenting satisfactory in all the stages in which it was evaluated. These results indicate that the established bank remained stable over 10 months and is apt to be used as a prototype for a WCB in compliance with GMP. |
| publishDate |
2017 |
| dc.date.none.fl_str_mv |
2017-12-12T18:15:18Z 2017-12-12T18:15:18Z 2017-02-23 |
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info:eu-repo/semantics/publishedVersion |
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info:eu-repo/semantics/masterThesis |
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masterThesis |
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publishedVersion |
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FARIA, Surian Guerios. Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase. 2017. 134 f. Dissertação (Mestrado em Engenharia Biomédica) - Universidade Tecnológica Federal do Paraná, Curitiba, 2017. http://repositorio.utfpr.edu.br/jspui/handle/1/2729 |
| identifier_str_mv |
FARIA, Surian Guerios. Estabelecimento e caracterização de um banco de células de trabalho para produção da enzima Taq DNA polimerase. 2017. 134 f. Dissertação (Mestrado em Engenharia Biomédica) - Universidade Tecnológica Federal do Paraná, Curitiba, 2017. |
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http://repositorio.utfpr.edu.br/jspui/handle/1/2729 |
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por |
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application/pdf |
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Universidade Tecnológica Federal do Paraná Curitiba Brasil Programa de Pós-Graduação em Engenharia Biomédica UTFPR |
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Universidade Tecnológica Federal do Paraná Curitiba Brasil Programa de Pós-Graduação em Engenharia Biomédica UTFPR |
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Repositório Institucional da UTFPR (da Universidade Tecnológica Federal do Paraná (RIUT)) - Universidade Tecnológica Federal do Paraná (UTFPR) |
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