PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies

Detalhes bibliográficos
Autor(a) principal: Rodrigues, Bruno Daniel Lopes
Data de Publicação: 2023
Tipo de documento: Dissertação
Idioma: eng
Título da fonte: Repositório Científico de Acesso Aberto de Portugal (Repositórios Cientìficos)
Texto Completo: http://hdl.handle.net/10400.6/13610
Resumo: Currently, the metalloprotease "A disintegrin and metalloproteinase 17" (ADAM17) has been gaining prominence due to its important action in signalling pathways where the soluble interleukin receptor - 6 (sIL-6R), the epidermal growth factor receptor (EGF-R) and the tumour necrosis factor alfa receptor (TNF-aR) participate, establishing ADAM17 as an attractive target in cancer therapy and infectious diseases. Thus, due to the high specificity of antibodies to recognize a particular epitope, it was possible to develop an anti-ADAM17 antibody, named MEDI3622, which has been shown to have the ability to specifically block the activity of ADAM17. Furthermore, the messenger Ribonucleic Acid (mRNA) has been showing great potential and applicability in several areas, namely in passive immunization, by the in vivo expression of antibodies, making mRNA a highly attractive method. Thus, in the present work, an mRNA sequence was prepared with the coding sequence of MEDI3622 for expression of this anti-ADAM17 antibody. Therefore, given the great therapeutic potential of mRNA, the high demand from the biopharmaceutical industry and the need to obtain it in a stable and pure form, it is important to optimize the production and purification processes of this biomolecule. The cryogels have emerged as a new alternative to conventional particulate chromatographic media for the purification of high molecular weight molecules, and their potential has already been demonstrated in the purification of the supercoiled isoform of plasmidic deoxyribonucleic acid (pDNA). Cryogels also have a supermacroporous structure that allows for facilitated diffusion, high flow rates, and high capacity. Currently, the strategy of choice for mRNA purification is affinity chromatography, using nucleotides as ligands, whose adenine and thymine base pairing specificity promotes highly selective and specific interactions. Thus, the aim of this work was to synthesize thymine-functionalized cryogels to purify the mRNA sequence produced by in vitro transcription, that encodes the anti-ADAM17 antibody MEDI3622. To this end, the ligand 1-(2-propenyl) thymine (ProT) was synthesized and characterized by nuclear magnetic resonance (NMR), the cryogels were subsequently prepared based on the monomer 2-hydroxyethyl methacrylate (HEMA), by copolymerization of the monomers HEMA and ProT, with different mass ratios of ProT and subjected to cryogenic treatment. The cryogels were characterized by scanning electron microscopy (SEM), energy dispersive X-ray analysis (EDXA), and rehydration capacity tests. Subsequently, to evaluate the behaviour of poly-thymine cryogels, purification tests were first performed under different conditions, varying the ionic strength, the type of salt (sodium chloride (NaCl) or ammonium sulphate ((NH4)2SO4)) and the pH in the mobile phase, taking advantage of the affinity between ProT ligands and adenines present in low molecular weight RNA (LMW RNA) used as a model sample, aiming to identify the best conditions under which binding and elution occurred. In the second phase, having already optimized the binding and elution conditions, the ability of cryogels to purify the mRNA was tested. In this phase, the NaCl concentration in the elution buffers was varied in order to achieve the separation between mRNA and pDNA used for its production. As the main results, the synthesis of the ligand 1-(2-propenyl) thymine was successfully achieved. Furthermore, in this task, it was also possible to isolate the unreacted thymine and a by-product of the reaction in which di-alkylation of thymine occurred (1,3-bis(2- propenyl) thymine). The fact that it was possible to isolate these two compounds makes the present work fit in with the principles of circular economy, reducing the costs of the synthesis of the ligand by reusing the isolated thymine, while eliminating the waste of by-products by the possibility of using di-alkylated thymine as a cross-linking agent instead of N, N'-Methylenebisacrylamide. However, traces of a second by-product (3-(2- propenyl) thymine) were found, and it was not possible to fully isolate the ligand of interest due to its structural similarity to this by-product, thus the isolation step needs to be optimized in the future. Regarding the characterization of the cryogels, the functionalized ones did not show significant changes in rehydration capacity compared to the non-functionalized one. Differences in morphology were visualized, which may denote the presence of the ligand in the polymeric matrix of the cryogels. Also, they may have resulted from the conditions used in the synthesis process of cryogels. Furthermore, through the EDXA, it was possible to confirm that there was functionalization of the cryogels, however, this method is not the most indicated for this type of confirmation, other methods, such as elemental analysis and solid-state NMR, can be used in the future to corroborate the results at the functionalization level. The results of the chromatographic assays demonstrate that the ProT functionalized cryogels were able to bind and elute mRNA and pDNA. Moreover, they showed potential to separate pDNA and mRNA, demonstrating a higher affinity for mRNA. The control cryogel (with no ProT ligand incorporated) also demonstrated the ability to bind and elute both mRNA and pDNA, however, it showed no aptitude to separate these two biomolecules. Thus, ProT functionalized cryogels appear to be a novel approach to overcoming challenges in mRNA purification.
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spelling PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodiesAdam17CriogéisCromatografia de AfinidadeMedi3622MrnaTiminaDomínio/Área Científica::Engenharia e Tecnologia::BioquímicaCurrently, the metalloprotease "A disintegrin and metalloproteinase 17" (ADAM17) has been gaining prominence due to its important action in signalling pathways where the soluble interleukin receptor - 6 (sIL-6R), the epidermal growth factor receptor (EGF-R) and the tumour necrosis factor alfa receptor (TNF-aR) participate, establishing ADAM17 as an attractive target in cancer therapy and infectious diseases. Thus, due to the high specificity of antibodies to recognize a particular epitope, it was possible to develop an anti-ADAM17 antibody, named MEDI3622, which has been shown to have the ability to specifically block the activity of ADAM17. Furthermore, the messenger Ribonucleic Acid (mRNA) has been showing great potential and applicability in several areas, namely in passive immunization, by the in vivo expression of antibodies, making mRNA a highly attractive method. Thus, in the present work, an mRNA sequence was prepared with the coding sequence of MEDI3622 for expression of this anti-ADAM17 antibody. Therefore, given the great therapeutic potential of mRNA, the high demand from the biopharmaceutical industry and the need to obtain it in a stable and pure form, it is important to optimize the production and purification processes of this biomolecule. The cryogels have emerged as a new alternative to conventional particulate chromatographic media for the purification of high molecular weight molecules, and their potential has already been demonstrated in the purification of the supercoiled isoform of plasmidic deoxyribonucleic acid (pDNA). Cryogels also have a supermacroporous structure that allows for facilitated diffusion, high flow rates, and high capacity. Currently, the strategy of choice for mRNA purification is affinity chromatography, using nucleotides as ligands, whose adenine and thymine base pairing specificity promotes highly selective and specific interactions. Thus, the aim of this work was to synthesize thymine-functionalized cryogels to purify the mRNA sequence produced by in vitro transcription, that encodes the anti-ADAM17 antibody MEDI3622. To this end, the ligand 1-(2-propenyl) thymine (ProT) was synthesized and characterized by nuclear magnetic resonance (NMR), the cryogels were subsequently prepared based on the monomer 2-hydroxyethyl methacrylate (HEMA), by copolymerization of the monomers HEMA and ProT, with different mass ratios of ProT and subjected to cryogenic treatment. The cryogels were characterized by scanning electron microscopy (SEM), energy dispersive X-ray analysis (EDXA), and rehydration capacity tests. Subsequently, to evaluate the behaviour of poly-thymine cryogels, purification tests were first performed under different conditions, varying the ionic strength, the type of salt (sodium chloride (NaCl) or ammonium sulphate ((NH4)2SO4)) and the pH in the mobile phase, taking advantage of the affinity between ProT ligands and adenines present in low molecular weight RNA (LMW RNA) used as a model sample, aiming to identify the best conditions under which binding and elution occurred. In the second phase, having already optimized the binding and elution conditions, the ability of cryogels to purify the mRNA was tested. In this phase, the NaCl concentration in the elution buffers was varied in order to achieve the separation between mRNA and pDNA used for its production. As the main results, the synthesis of the ligand 1-(2-propenyl) thymine was successfully achieved. Furthermore, in this task, it was also possible to isolate the unreacted thymine and a by-product of the reaction in which di-alkylation of thymine occurred (1,3-bis(2- propenyl) thymine). The fact that it was possible to isolate these two compounds makes the present work fit in with the principles of circular economy, reducing the costs of the synthesis of the ligand by reusing the isolated thymine, while eliminating the waste of by-products by the possibility of using di-alkylated thymine as a cross-linking agent instead of N, N'-Methylenebisacrylamide. However, traces of a second by-product (3-(2- propenyl) thymine) were found, and it was not possible to fully isolate the ligand of interest due to its structural similarity to this by-product, thus the isolation step needs to be optimized in the future. Regarding the characterization of the cryogels, the functionalized ones did not show significant changes in rehydration capacity compared to the non-functionalized one. Differences in morphology were visualized, which may denote the presence of the ligand in the polymeric matrix of the cryogels. Also, they may have resulted from the conditions used in the synthesis process of cryogels. Furthermore, through the EDXA, it was possible to confirm that there was functionalization of the cryogels, however, this method is not the most indicated for this type of confirmation, other methods, such as elemental analysis and solid-state NMR, can be used in the future to corroborate the results at the functionalization level. The results of the chromatographic assays demonstrate that the ProT functionalized cryogels were able to bind and elute mRNA and pDNA. Moreover, they showed potential to separate pDNA and mRNA, demonstrating a higher affinity for mRNA. The control cryogel (with no ProT ligand incorporated) also demonstrated the ability to bind and elute both mRNA and pDNA, however, it showed no aptitude to separate these two biomolecules. Thus, ProT functionalized cryogels appear to be a novel approach to overcoming challenges in mRNA purification.A metaloprotease “A Desintegrin And Metalloproteinase 17” (ADAM17) tem vindo a ganhar destaque devido à sua importante ação nas vias de sinalização onde participa, particularmente na interação com o recetor solúvel da interleucina - 6 (soluble interleukin receptor – 6, sIL-6R), o recetor do fator de crescimento epidérmico (Epithermal Growth Factor Receptor, EGF-R) e o recetor do fator de necrose tumoral (Receptor of Tumour Necrosis Factor, TNF-aR), estabelecendo a ADAM17 como um alvo atrativo na terapêutica contra o cancro e doenças infeciosas. Assim, devido à grande especificidade dos anticorpos para reconhecer um determinado epítopo, foi possível desenvolver um anticorpo anti-ADAM17, denominado de MEDI3622, que demonstrou ter a habilidade de bloquear especificamente a atividade da ADAM17. Além disso, o ácido ribonucleico mensageiro (mRNA) tem vindo a demonstrar grande potencial e aplicabilidade em diversas áreas, nomeadamente na imunização passiva, através da expressão in vivo de anticorpos. Deste modo, no presente trabalho foi preparado mRNA com a sequência codificante do MEDI3622 para expressão deste anticorpo antiADAM17. Assim, dado o grande potencial terapêutico do mRNA, a elevada procura por parte da indústria biofarmacêutica e a necessidade de ser obtido na forma estável e pura, tornase urgente otimizar os processos de produção e purificação desta biomolécula. Os criogeis surgiram como uma nova alternativa aos suportes cromatográficos particulados convencionais para a purificação de moléculas com elevado peso molecular, tendo já sido demonstrado o seu potencial na purificação da isoforma superenrolada do ácido desoxirribonucleico plasmídico (pDNA). Devido à sua estrutura supermacroporosa, os criogeis permitem difusão facilitada, altas taxas de fluxo e alta capacidade. Atualmente, a estratégia de eleição para a purificação do mRNA é a cromatografia de afinidade, através do uso de nucleótidos como ligandos, cuja especificidade do emparelhamento das bases adenina e timina promove interações altamente seletivas e específicas. Deste modo, o objetivo deste trabalho foi sintetizar criogéis funcionalizados com timina, para purificar a sequência de mRNA produzida por transcrição in vitro que codifica o anticorpo anti-ADAM17, o MEDI3622. Para isso, o ligando 1-(2-propenil) Timina (ProT) foi sintetizado e caracterizado por ressonância magnética nuclear (RMN), sendo posteriormente preparados criogeis à base do monómero 2-hidroxietilmetacrilato (HEMA), por copolimerização dos monómeros HEMA e ProT, com diferentes proporções mássicas de ProT e submetidos a um tratamento criogénico. Os criogeis foram caracterizados por microscopia eletrónica de varrimento (scanning electron microscopy, SEM), análise de energia dispersiva de raios-X (energy dispersive X-ray analysis, EDXA), e testes de capacidade de reidratação. Posteriormente, para avaliação do comportamento dos criogeis poli-Timina, foram realizados ensaios de purificação em diferentes condições, variando a força iónica, o tipo de sal (cloreto de sódio (NaCl) ou sulfato de amónio ((NH4)2SO4)) e o pH na fase móvel, tirando partido da afinidade entre os ligandos ProT e as adeninas presentes em amostras de low molecular weight RNA (LMW RNA) como moléculas modelo, visando identificar as melhores condições em que ocorreria ligação e eluição. Numa segunda fase, após a otimização destas condições, testou-se a capacidade dos criogeis poli-Timina para purificar o mRNA, por variação da concentração de NaCl no eluente, de forma a promover a separação entre o mRNA e pDNA utilizado na sua produção. Como principais resultados, destaca-se a síntese do ligando 1-(2-propenil) timina que foi bem-sucedida. Além disso, nesta tarefa foi ainda possível isolar a timina que não reagiu e um subproduto da reação no qual ocorreu a di-alquilação da timina (1,3-bis(2-propenil) timina). O isolamento destes dois compostos mostra que o presente trabalho se enquadra nos princípios da economia circular, reduzindo os custos da síntese do ligando, permitindo a reutilização da timina, ao mesmo tempo que são eliminados desperdícios de subprodutos através da possibilidade do uso da timina di-alquilada como agente de reticulação, ao invés da N, N'-metilenobisacrilamida. Contudo, encontraram-se vestígios de um segundo subproduto (3-(2-propenil) timina), não tendo sido possível isolar totalmente o ligando de interesse devido à sua semelhança estrutural com este subproduto, sendo necessário otimizar o passo de isolamento no futuro. Relativamente à caracterização dos criogéis, observou-se que os suportes funcionalizados não apresentaram alterações significativas na capacidade de reidratação, em comparação com o não funcionalizado. Além disso, visualizaram-se diferenças ao nível da morfologia entre os criogéis poli-Timina e o controlo, podendo estar relacionadas com a presença do ligando na matriz polimérica dos criogéis. Estas diferenças podem, ainda, ter resultado das condições utilizadas no processo de síntese dos criogéis. Através de EDXA foi possível confirmar que houve funcionalização dos criogéis, contudo este método não é o mais indicado devido à sua limitada sensibilidade, sendo desejável a utilização de outros métodos, como análise elementar e RMN em estado-sólido, para confirmar os resultados ao nível da funcionalização. Os resultados dos ensaios cromatográficos demonstraram que os criogéis funcionalizados com ProT conseguiram ligar e eluir o mRNA e o pDNA, apresentando maior afinidade para o mRNA, e portanto, potencial para separar estas biomoléculas. O criogel de controlo também demonstrou capacidade para ligar e eluir tanto o mRNA como o pDNA, contudo não apresentou seletividade para separar estas duas biomoléculas. Assim, os criogeis funcionalizados com ProT parecem ser uma abordagem inovadora para superar alguns dos desafios na purificação do mRNA.Tomaz, Cândida Ascensão TeixeiraSousa, Fani Pereira deuBibliorumRodrigues, Bruno Daniel Lopes2023-03-072023-01-312024-01-31T00:00:00Z2023-03-07T00:00:00Zinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesisapplication/pdfhttp://hdl.handle.net/10400.6/13610TID:203381769enginfo:eu-repo/semantics/embargoedAccessreponame:Repositório Científico de Acesso Aberto de Portugal (Repositórios Cientìficos)instname:Agência para a Sociedade do Conhecimento (UMIC) - FCT - Sociedade da Informaçãoinstacron:RCAAP2023-12-15T09:57:16Zoai:ubibliorum.ubi.pt:10400.6/13610Portal AgregadorONGhttps://www.rcaap.pt/oai/openaireopendoar:71602024-03-20T00:53:00.775562Repositório Científico de Acesso Aberto de Portugal (Repositórios Cientìficos) - Agência para a Sociedade do Conhecimento (UMIC) - FCT - Sociedade da Informaçãofalse
dc.title.none.fl_str_mv PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
title PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
spellingShingle PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
Rodrigues, Bruno Daniel Lopes
Adam17
Criogéis
Cromatografia de Afinidade
Medi3622
Mrna
Timina
Domínio/Área Científica::Engenharia e Tecnologia::Bioquímica
title_short PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
title_full PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
title_fullStr PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
title_full_unstemmed PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
title_sort PolyThymine cryogels as a novel approach to the purification of mRNA encoding anti- ADAM17 antibodies
author Rodrigues, Bruno Daniel Lopes
author_facet Rodrigues, Bruno Daniel Lopes
author_role author
dc.contributor.none.fl_str_mv Tomaz, Cândida Ascensão Teixeira
Sousa, Fani Pereira de
uBibliorum
dc.contributor.author.fl_str_mv Rodrigues, Bruno Daniel Lopes
dc.subject.por.fl_str_mv Adam17
Criogéis
Cromatografia de Afinidade
Medi3622
Mrna
Timina
Domínio/Área Científica::Engenharia e Tecnologia::Bioquímica
topic Adam17
Criogéis
Cromatografia de Afinidade
Medi3622
Mrna
Timina
Domínio/Área Científica::Engenharia e Tecnologia::Bioquímica
description Currently, the metalloprotease "A disintegrin and metalloproteinase 17" (ADAM17) has been gaining prominence due to its important action in signalling pathways where the soluble interleukin receptor - 6 (sIL-6R), the epidermal growth factor receptor (EGF-R) and the tumour necrosis factor alfa receptor (TNF-aR) participate, establishing ADAM17 as an attractive target in cancer therapy and infectious diseases. Thus, due to the high specificity of antibodies to recognize a particular epitope, it was possible to develop an anti-ADAM17 antibody, named MEDI3622, which has been shown to have the ability to specifically block the activity of ADAM17. Furthermore, the messenger Ribonucleic Acid (mRNA) has been showing great potential and applicability in several areas, namely in passive immunization, by the in vivo expression of antibodies, making mRNA a highly attractive method. Thus, in the present work, an mRNA sequence was prepared with the coding sequence of MEDI3622 for expression of this anti-ADAM17 antibody. Therefore, given the great therapeutic potential of mRNA, the high demand from the biopharmaceutical industry and the need to obtain it in a stable and pure form, it is important to optimize the production and purification processes of this biomolecule. The cryogels have emerged as a new alternative to conventional particulate chromatographic media for the purification of high molecular weight molecules, and their potential has already been demonstrated in the purification of the supercoiled isoform of plasmidic deoxyribonucleic acid (pDNA). Cryogels also have a supermacroporous structure that allows for facilitated diffusion, high flow rates, and high capacity. Currently, the strategy of choice for mRNA purification is affinity chromatography, using nucleotides as ligands, whose adenine and thymine base pairing specificity promotes highly selective and specific interactions. Thus, the aim of this work was to synthesize thymine-functionalized cryogels to purify the mRNA sequence produced by in vitro transcription, that encodes the anti-ADAM17 antibody MEDI3622. To this end, the ligand 1-(2-propenyl) thymine (ProT) was synthesized and characterized by nuclear magnetic resonance (NMR), the cryogels were subsequently prepared based on the monomer 2-hydroxyethyl methacrylate (HEMA), by copolymerization of the monomers HEMA and ProT, with different mass ratios of ProT and subjected to cryogenic treatment. The cryogels were characterized by scanning electron microscopy (SEM), energy dispersive X-ray analysis (EDXA), and rehydration capacity tests. Subsequently, to evaluate the behaviour of poly-thymine cryogels, purification tests were first performed under different conditions, varying the ionic strength, the type of salt (sodium chloride (NaCl) or ammonium sulphate ((NH4)2SO4)) and the pH in the mobile phase, taking advantage of the affinity between ProT ligands and adenines present in low molecular weight RNA (LMW RNA) used as a model sample, aiming to identify the best conditions under which binding and elution occurred. In the second phase, having already optimized the binding and elution conditions, the ability of cryogels to purify the mRNA was tested. In this phase, the NaCl concentration in the elution buffers was varied in order to achieve the separation between mRNA and pDNA used for its production. As the main results, the synthesis of the ligand 1-(2-propenyl) thymine was successfully achieved. Furthermore, in this task, it was also possible to isolate the unreacted thymine and a by-product of the reaction in which di-alkylation of thymine occurred (1,3-bis(2- propenyl) thymine). The fact that it was possible to isolate these two compounds makes the present work fit in with the principles of circular economy, reducing the costs of the synthesis of the ligand by reusing the isolated thymine, while eliminating the waste of by-products by the possibility of using di-alkylated thymine as a cross-linking agent instead of N, N'-Methylenebisacrylamide. However, traces of a second by-product (3-(2- propenyl) thymine) were found, and it was not possible to fully isolate the ligand of interest due to its structural similarity to this by-product, thus the isolation step needs to be optimized in the future. Regarding the characterization of the cryogels, the functionalized ones did not show significant changes in rehydration capacity compared to the non-functionalized one. Differences in morphology were visualized, which may denote the presence of the ligand in the polymeric matrix of the cryogels. Also, they may have resulted from the conditions used in the synthesis process of cryogels. Furthermore, through the EDXA, it was possible to confirm that there was functionalization of the cryogels, however, this method is not the most indicated for this type of confirmation, other methods, such as elemental analysis and solid-state NMR, can be used in the future to corroborate the results at the functionalization level. The results of the chromatographic assays demonstrate that the ProT functionalized cryogels were able to bind and elute mRNA and pDNA. Moreover, they showed potential to separate pDNA and mRNA, demonstrating a higher affinity for mRNA. The control cryogel (with no ProT ligand incorporated) also demonstrated the ability to bind and elute both mRNA and pDNA, however, it showed no aptitude to separate these two biomolecules. Thus, ProT functionalized cryogels appear to be a novel approach to overcoming challenges in mRNA purification.
publishDate 2023
dc.date.none.fl_str_mv 2023-03-07
2023-01-31
2023-03-07T00:00:00Z
2024-01-31T00:00:00Z
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