Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.

Detalhes bibliográficos
Autor(a) principal: Silva, Gracinda Marina Castelo da
Data de Publicação: 2004
Tipo de documento: Dissertação
Idioma: por
Título da fonte: Repositório Institucional da UFSCAR
Texto Completo: https://repositorio.ufscar.br/handle/ufscar/4059
Resumo: Disintegrins are proteins present in the poison of serpents that have been calling the pharmaceutical industry attention due to their capacity to prevent the progression of cancerous cells. A receiving key-protein called integrin addresses the formation of new blood vessels instructing the tumor cells to increase and spread. The disintegrin acts as an inhibitor that blocks this interaction. In order to produce substantial amounts of disintegrin in industrial scale, its expression in CHO-K1 cells was carried out by cloning the characteristic DNA extracted from the poison producing glands of the serpent Agkistrodon contortrix laticinctus. Usually CHO-K1 cells are cultivated in medium containing bovine fetal serum. However, its presence in the cultivation medium hinders the stages of detection, extraction and purification of the protein of interest. The objective of this work was to study the CHOZMD cell growth and the desintegrin production in serum free medium, as well as to develope a methodology for the detection and quantification of the disintegrin present in the medium. The cultivations were carried in culture bottles of 25cm2, 75cm2 and 150cm2 and later in spinner flask with a volume of 500mL, incubated with an amount of CO2 controlled in 10% v/v, pH between 7.0 to 7.4, a temperature of 37 °C, under agitation conditions. The cells were cultivated in the presence of the microcarrrier Pronectin F which enables the attainment of high cell concentration. The culture media DMEM and CHO-S-SFM II were used in the cultivations by means of a gradual adaptation process for a serum free medium, through the reduction of DMEM+serum proportion at each change, until that it was totally replaced by the serum free medium. The cells were maintained in 100% serum free medium during 6h with the withdrawal of 250 ml after 3 h and of the remaining volume after 6h of cultivation. For the detection of the disintegrin, the samples were initially filtered in Milipore filter, then concentrated in ultra filter Amicon and finally centrifuged in membranes Centriprep and Centricon. The disintegrin, protein of ~70kDa, present in the treated samples was detected using Bio Dot equipment with nitrocelulose membrane incubated with specific antibodies. The samples were applied in ion exchange column and the fractions obtained applied in nitrocelulose membrane. In the cultivations carried out in serum free medium with the microcarrier Pronectin F a maximum cell concentration of 1.74.106 cel.ml-1 was reached, which is slightly inferior to the value reached in the cultivations in medium containing serum (2.7.106 cel.mL-1). However, concerning product formation, the immunodetecion results revealed the presence of the disintegrin in the cultivations carried out with serum free medium. Cultivations carried out in spinner flask, with a volume of 200mL and using microcarrier Citodex 1 and medium supplemented with 1% hemolymph (v/v) presented maximum cell concentration of 2.6.106 cel.mL-1. The detection method developed was effective in the identification of the target protein in the samples from the cultivation medium containing hemolymph. Preliminary tests demonstrated loss of protein might be related to gradual degradation in cultivation medium or retention in ion exchange column.
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spelling Silva, Gracinda Marina Castelo daZangirolami, Teresa Cristinahttp://lattes.cnpq.br/4546701843297248http://genos.cnpq.br:12010/dwlattes/owa/prc_imp_cv_int?f_cod=K4775040Y3ed8b5ad1-c7ad-4b33-adcb-a8e3a2ee1c592016-06-02T19:56:41Z2005-01-062016-06-02T19:56:41Z2004-06-25SILVA, Gracinda Marina Castelo da. Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.. 2004. 153 f. Dissertação (Mestrado em Ciências Exatas e da Terra) - Universidade Federal de São Carlos, São Carlos, 2004.https://repositorio.ufscar.br/handle/ufscar/4059Disintegrins are proteins present in the poison of serpents that have been calling the pharmaceutical industry attention due to their capacity to prevent the progression of cancerous cells. A receiving key-protein called integrin addresses the formation of new blood vessels instructing the tumor cells to increase and spread. The disintegrin acts as an inhibitor that blocks this interaction. In order to produce substantial amounts of disintegrin in industrial scale, its expression in CHO-K1 cells was carried out by cloning the characteristic DNA extracted from the poison producing glands of the serpent Agkistrodon contortrix laticinctus. Usually CHO-K1 cells are cultivated in medium containing bovine fetal serum. However, its presence in the cultivation medium hinders the stages of detection, extraction and purification of the protein of interest. The objective of this work was to study the CHOZMD cell growth and the desintegrin production in serum free medium, as well as to develope a methodology for the detection and quantification of the disintegrin present in the medium. The cultivations were carried in culture bottles of 25cm2, 75cm2 and 150cm2 and later in spinner flask with a volume of 500mL, incubated with an amount of CO2 controlled in 10% v/v, pH between 7.0 to 7.4, a temperature of 37 °C, under agitation conditions. The cells were cultivated in the presence of the microcarrrier Pronectin F which enables the attainment of high cell concentration. The culture media DMEM and CHO-S-SFM II were used in the cultivations by means of a gradual adaptation process for a serum free medium, through the reduction of DMEM+serum proportion at each change, until that it was totally replaced by the serum free medium. The cells were maintained in 100% serum free medium during 6h with the withdrawal of 250 ml after 3 h and of the remaining volume after 6h of cultivation. For the detection of the disintegrin, the samples were initially filtered in Milipore filter, then concentrated in ultra filter Amicon and finally centrifuged in membranes Centriprep and Centricon. The disintegrin, protein of ~70kDa, present in the treated samples was detected using Bio Dot equipment with nitrocelulose membrane incubated with specific antibodies. The samples were applied in ion exchange column and the fractions obtained applied in nitrocelulose membrane. In the cultivations carried out in serum free medium with the microcarrier Pronectin F a maximum cell concentration of 1.74.106 cel.ml-1 was reached, which is slightly inferior to the value reached in the cultivations in medium containing serum (2.7.106 cel.mL-1). However, concerning product formation, the immunodetecion results revealed the presence of the disintegrin in the cultivations carried out with serum free medium. Cultivations carried out in spinner flask, with a volume of 200mL and using microcarrier Citodex 1 and medium supplemented with 1% hemolymph (v/v) presented maximum cell concentration of 2.6.106 cel.mL-1. The detection method developed was effective in the identification of the target protein in the samples from the cultivation medium containing hemolymph. Preliminary tests demonstrated loss of protein might be related to gradual degradation in cultivation medium or retention in ion exchange column.Desintegrinas são proteínas presentes no veneno de serpentes que têm despertado interesse da indústria farmacêutica por sua capacidade de impedir a progressão de células cancerígenas. Uma proteína-chave receptora chamada integrina direciona a formação de novos vasos sangüíneos instruindo as células do tumor a crescerem e se espalharem. A desintegrina atua como um inibidor que bloqueia essa interação. Para que quantidades substanciais de desintegrina possam ser produzidas em escala industrial, realizou-se a expressão da mesma em células CHO-K1, produzidas por clonagem do ADN característico retirado das glândulas produtoras do veneno da serpente Agkistrodon contortrix laticinctus. Normalmente as células CHO-K1 são cultivadas em meio contendo soro fetal bovino. No entanto, a presença do mesmo no meio de cultivo dificulta as etapas de detecção, extração e purificação da proteína de interesse. O objetivo deste trabalho foi estudar o crescimento de células CHO-K1 e a produção da desintegrina em meio livre de soro, assim como desenvolver uma metodologia para a detecção e quantificação da desintegrina presente no meio. Os cultivos foram realizados em garrafas de cultura de 25cm2, 75cm2 e 150cm2 e posteriormente em frasco spinner com um volume de 500mL, incubados em estufa com uma quantidade de CO2 controlada em 10% v/v, pH entre 7,0 a 7,4, a uma temperatura de 37 °C em condições de agitação brandas. As células foram cultivadas na presença do microcarrregador sólido Pronectin F, que possibilita a obtenção de uma alta concentração de células. Os meios de cultura DMEM e CHO-S-SFM II foram utilizados nos cultivos por um processo de adaptação gradual para um meio livre de soro, reduzindo-se a proporção de meio com soro a cada troca, até que fosse totalmente substituído para o meio livre de soro. As células foram mantidas em meio 100% livre de soro durante 6 h com a retirada de 250 ml após 3 h e o restante após 6 h de cultivo. Para a detecção da desintegrina, as amostras foram primeiramente filtradas em filtro Millipore e o filtrado concentrado em ultrafiltro Amicon e centrifugadas em membranas Centriprep e Centricon. A desintegrina, proteína de ~70KDa presente nas amostras tratadas, foi detectada utilizando-se equipamento Bio Dot em membrana de nitrocelulose incubada com anticorpos específicos. As amostras foram aplicadas em coluna de troca iônica e as frações obtidas aplicadas em membrana de nitrocelulose. Nos cultivos realizados em meio livre de soro com o microcarregador Pronectin F foi atingida uma concentração celular máxima de 1,74.106 cel.ml-1, a qual é ligeiramente inferior ao valor alcançado nos cultivos em meio contendo soro (2,7.106 cel.mL-1). Entretanto no que se refere à formação do produto o resultado na membrana de nitrocelulose evidencia a presença da desintegrina no meio de cultivo livre de soro. Cultivos realizados em meio suplementado com 1% v/v de hemolinfa apresentaram concentração celular máxima de 2,6. 106 cel.mL-1 em frasco Spinner, com um volume de 200mL e utilizando microcarregador Citodex 1. O método de detecção desenvolvido foi efetivo na identificação da proteína de interesse nas amostras retiradas do cultivo em meio contendo hemolinfa. Testes preliminares demonstraram que a proteína pode estar degradando gradativamente em meio de cultivo ou ficando retida na coluna de troca iônica.Financiadora de Estudos e Projetosapplication/pdfporUniversidade Federal de São CarlosPrograma de Pós-Graduação em Engenharia Química - PPGEQUFSCarBRBiotecnologiaCélulas CHO-K1Proteína recombinanteEngenharia bioquímicaENGENHARIAS::ENGENHARIA QUIMICAContribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.info:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesis-1-14c81169f-86ab-4df0-8284-9cb6516960a4info:eu-repo/semantics/openAccessreponame:Repositório Institucional da UFSCARinstname:Universidade Federal de São Carlos (UFSCAR)instacron:UFSCARORIGINALDissGMCS.pdfapplication/pdf2717580https://repositorio.ufscar.br/bitstream/ufscar/4059/1/DissGMCS.pdfff4f01b1bf27d70757eb37ee1960edefMD51THUMBNAILDissGMCS.pdf.jpgDissGMCS.pdf.jpgIM Thumbnailimage/jpeg7829https://repositorio.ufscar.br/bitstream/ufscar/4059/2/DissGMCS.pdf.jpge906b8113245a537319132f371ee3a4aMD52ufscar/40592023-09-18 18:30:59.444oai:repositorio.ufscar.br:ufscar/4059Repositório InstitucionalPUBhttps://repositorio.ufscar.br/oai/requestopendoar:43222023-09-18T18:30:59Repositório Institucional da UFSCAR - Universidade Federal de São Carlos (UFSCAR)false
dc.title.por.fl_str_mv Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
title Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
spellingShingle Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
Silva, Gracinda Marina Castelo da
Biotecnologia
Células CHO-K1
Proteína recombinante
Engenharia bioquímica
ENGENHARIAS::ENGENHARIA QUIMICA
title_short Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
title_full Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
title_fullStr Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
title_full_unstemmed Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
title_sort Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.
author Silva, Gracinda Marina Castelo da
author_facet Silva, Gracinda Marina Castelo da
author_role author
dc.contributor.authorlattes.por.fl_str_mv http://genos.cnpq.br:12010/dwlattes/owa/prc_imp_cv_int?f_cod=K4775040Y3
dc.contributor.author.fl_str_mv Silva, Gracinda Marina Castelo da
dc.contributor.advisor1.fl_str_mv Zangirolami, Teresa Cristina
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/4546701843297248
dc.contributor.authorID.fl_str_mv ed8b5ad1-c7ad-4b33-adcb-a8e3a2ee1c59
contributor_str_mv Zangirolami, Teresa Cristina
dc.subject.por.fl_str_mv Biotecnologia
Células CHO-K1
Proteína recombinante
Engenharia bioquímica
topic Biotecnologia
Células CHO-K1
Proteína recombinante
Engenharia bioquímica
ENGENHARIAS::ENGENHARIA QUIMICA
dc.subject.cnpq.fl_str_mv ENGENHARIAS::ENGENHARIA QUIMICA
description Disintegrins are proteins present in the poison of serpents that have been calling the pharmaceutical industry attention due to their capacity to prevent the progression of cancerous cells. A receiving key-protein called integrin addresses the formation of new blood vessels instructing the tumor cells to increase and spread. The disintegrin acts as an inhibitor that blocks this interaction. In order to produce substantial amounts of disintegrin in industrial scale, its expression in CHO-K1 cells was carried out by cloning the characteristic DNA extracted from the poison producing glands of the serpent Agkistrodon contortrix laticinctus. Usually CHO-K1 cells are cultivated in medium containing bovine fetal serum. However, its presence in the cultivation medium hinders the stages of detection, extraction and purification of the protein of interest. The objective of this work was to study the CHOZMD cell growth and the desintegrin production in serum free medium, as well as to develope a methodology for the detection and quantification of the disintegrin present in the medium. The cultivations were carried in culture bottles of 25cm2, 75cm2 and 150cm2 and later in spinner flask with a volume of 500mL, incubated with an amount of CO2 controlled in 10% v/v, pH between 7.0 to 7.4, a temperature of 37 °C, under agitation conditions. The cells were cultivated in the presence of the microcarrrier Pronectin F which enables the attainment of high cell concentration. The culture media DMEM and CHO-S-SFM II were used in the cultivations by means of a gradual adaptation process for a serum free medium, through the reduction of DMEM+serum proportion at each change, until that it was totally replaced by the serum free medium. The cells were maintained in 100% serum free medium during 6h with the withdrawal of 250 ml after 3 h and of the remaining volume after 6h of cultivation. For the detection of the disintegrin, the samples were initially filtered in Milipore filter, then concentrated in ultra filter Amicon and finally centrifuged in membranes Centriprep and Centricon. The disintegrin, protein of ~70kDa, present in the treated samples was detected using Bio Dot equipment with nitrocelulose membrane incubated with specific antibodies. The samples were applied in ion exchange column and the fractions obtained applied in nitrocelulose membrane. In the cultivations carried out in serum free medium with the microcarrier Pronectin F a maximum cell concentration of 1.74.106 cel.ml-1 was reached, which is slightly inferior to the value reached in the cultivations in medium containing serum (2.7.106 cel.mL-1). However, concerning product formation, the immunodetecion results revealed the presence of the disintegrin in the cultivations carried out with serum free medium. Cultivations carried out in spinner flask, with a volume of 200mL and using microcarrier Citodex 1 and medium supplemented with 1% hemolymph (v/v) presented maximum cell concentration of 2.6.106 cel.mL-1. The detection method developed was effective in the identification of the target protein in the samples from the cultivation medium containing hemolymph. Preliminary tests demonstrated loss of protein might be related to gradual degradation in cultivation medium or retention in ion exchange column.
publishDate 2004
dc.date.issued.fl_str_mv 2004-06-25
dc.date.available.fl_str_mv 2005-01-06
2016-06-02T19:56:41Z
dc.date.accessioned.fl_str_mv 2016-06-02T19:56:41Z
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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 SILVA, Gracinda Marina Castelo da. Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.. 2004. 153 f. Dissertação (Mestrado em Ciências Exatas e da Terra) - Universidade Federal de São Carlos, São Carlos, 2004.
dc.identifier.uri.fl_str_mv https://repositorio.ufscar.br/handle/ufscar/4059
identifier_str_mv SILVA, Gracinda Marina Castelo da. Contribuição ao desenvolvimento de metodologia para detecção de desintegrina recombinante produzida em cultivos de células CHO-K1.. 2004. 153 f. Dissertação (Mestrado em Ciências Exatas e da Terra) - Universidade Federal de São Carlos, São Carlos, 2004.
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