Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica

Detalhes bibliográficos
Ano de defesa: 2010
Autor(a) principal: Oliveira, Altamir Fernandes De lattes
Orientador(a): Brigagão, Maísa Ribeiro Pereira Lima lattes
Banca de defesa: D'Assunção, Lázaro Moscardini, Florenzano, Fábio Herbst
Tipo de documento: Dissertação
Tipo de acesso: Acesso aberto
Idioma: por
Instituição de defesa: Universidade Federal de Alfenas
Programa de Pós-Graduação: Programa de Pós-Graduação em Química
Departamento: Instituto de Química
País: Brasil
Palavras-chave em Português:
Cinética de enzimas
Chaperonas Moleculares
Inibidores Enzimáticas
Área do conhecimento CNPq:
FISICO-QUIMICA::CINETICA QUIMICA E CATALISE
Link de acesso: https://repositorio.unifal-mg.edu.br/handle/123456789/723
Resumo: Protein disulfide isomerase (PDI, EC 5.3.4.1) belonging to the thioredoxin superfamily, is a thiol oxidoreductase that catalyzes the oxidation and reduction of thiols and intramolecular disulfide isomerization. This chaperone, such activity is dependent of cysteine located on the active sites, is present in the endoplasmic reticulum (ER) and / or plasma membrane of eukaryotic cells. Previous studies of the catalytic activity of PDI were performed using different pseudo-substrates, among them, the di-eosin-glutathione disulfide (Di-E-GSSG), described as a usefull tool for monitoring the disulfide reductase activity of PDI . In this work, the synthesis and chromatographic purification of Di-E-GSSG were performed and the purity of the probe was verified by high performance liquid chromatography (HPLC). The enzyme kinetics of the reductase activity of recombinant PDI isolated over Di-E-GSSG was studied, characterizing the main physicochemical parameters of the enzyme through the formation of the fluorescent monomer (λexc=521nm; λemi=542nm) eosin-reduced glutathione (E-GSH). The value of the Michaelis-Menten constant (Km) was found to be 520.5 ± 129.8 nM, the maximum velocity of catalysis (Vmáx) was determined as 1,637 ± 0.1526 nM.min-¹ and the catalytic constant (Kcat) found was 1.364 . 10-³.s-¹. Few chemical compounds able to inhibit catalytic activity of PDI were reported. Thus, to verify if stable free radical compounds display this activity were tested piperidine nitroxides as potential inhibitors of PDI. These compounds, which have antioxidant, anti-inflammatory and radioprotective properties are “scavengers” of different radical species, among them, thyil radicals. The nitroxide 4-hydroxy-2,2,6,6-tetrametilpiperidine-1-oxyl (Tempol) was a weak inhibitor of PDI reductase activity. However, three other nitroxides specifically synthesized for this study showed higher inhibition power, with a direct correlation between increasing the hydrophobicity of the chemical structures and inhibitory action. This ability was confirmed by assays with PDI found in human platelets, confirming the hypothesis that the nitroxides are candidates for new drugs to modulate cellular functions involving the PDI activity.
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spelling Oliveira, Altamir Fernandes Dehttp://lattes.cnpq.br/0963588859777460D'Assunção, Lázaro MoscardiniFlorenzano, Fábio HerbstBrigagão, Maísa Ribeiro Pereira Limahttp://lattes.cnpq.br/29743192709351112015-11-18T17:06:52Z2010-12-07OLIVEIRA, Altamir Fernandes de. Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica. 2010. 93 f. Dissertação (Mestrado em Química) - Universidade Federal de Alfenas, Alfenas, MG, 2010.https://repositorio.unifal-mg.edu.br/handle/123456789/723Protein disulfide isomerase (PDI, EC 5.3.4.1) belonging to the thioredoxin superfamily, is a thiol oxidoreductase that catalyzes the oxidation and reduction of thiols and intramolecular disulfide isomerization. This chaperone, such activity is dependent of cysteine located on the active sites, is present in the endoplasmic reticulum (ER) and / or plasma membrane of eukaryotic cells. Previous studies of the catalytic activity of PDI were performed using different pseudo-substrates, among them, the di-eosin-glutathione disulfide (Di-E-GSSG), described as a usefull tool for monitoring the disulfide reductase activity of PDI . In this work, the synthesis and chromatographic purification of Di-E-GSSG were performed and the purity of the probe was verified by high performance liquid chromatography (HPLC). The enzyme kinetics of the reductase activity of recombinant PDI isolated over Di-E-GSSG was studied, characterizing the main physicochemical parameters of the enzyme through the formation of the fluorescent monomer (λexc=521nm; λemi=542nm) eosin-reduced glutathione (E-GSH). The value of the Michaelis-Menten constant (Km) was found to be 520.5 ± 129.8 nM, the maximum velocity of catalysis (Vmáx) was determined as 1,637 ± 0.1526 nM.min-¹ and the catalytic constant (Kcat) found was 1.364 . 10-³.s-¹. Few chemical compounds able to inhibit catalytic activity of PDI were reported. Thus, to verify if stable free radical compounds display this activity were tested piperidine nitroxides as potential inhibitors of PDI. These compounds, which have antioxidant, anti-inflammatory and radioprotective properties are “scavengers” of different radical species, among them, thyil radicals. The nitroxide 4-hydroxy-2,2,6,6-tetrametilpiperidine-1-oxyl (Tempol) was a weak inhibitor of PDI reductase activity. However, three other nitroxides specifically synthesized for this study showed higher inhibition power, with a direct correlation between increasing the hydrophobicity of the chemical structures and inhibitory action. This ability was confirmed by assays with PDI found in human platelets, confirming the hypothesis that the nitroxides are candidates for new drugs to modulate cellular functions involving the PDI activity.A Proteína Dissulfeto Isomerase (PDI, E.C. 5.3.4.1), pertencente à superfamília das tiorredoxinas, é uma tiol oxidorredutase que catalisa a oxidação e redução de tióis e a isomerização de dissulfetos intramoleculares. Essa chaperona tem atividade dependente de cisteínas presentes nos sítios ativos, e está presente no retículo endoplasmático (RE) e/ou na membrana plasmática de células eucarióticas. Estudos anteriores da atividade catalítica de PDI foram realizados utilizando-se como pseudo-substratos, entre eles, a di-eosinaglutationa oxidada (Di-E-GSSG), que se mostrou ótima ferramenta para o monitoramento da atividade de dissulfeto redutase da PDI. Nesse trabalho, a síntese e purificação cromatográfica de Di-E-GSSG foram realizadas e a pureza da sonda foi verificada através de cromatografia líquida de alta performance (CLAE). A cinética enzimática da atividade redutase de PDI isolada recombinante sobre Di-E-GSSG foi estudada, caracterizando-se os principais parâmetros físico-químicos da enzima através da formação do monômero fluorescente (λexc=521nm; λemi=542 nm) eosina-glutationa reduzida (E-GSH). O valor da constante de Michaelis-Menten (Km) encontrado foi de 520,5±129,8 nM, a velocidade máxima de catálise (Vmáx) foi determinada como 1,637±0,1526 nM.min-¹ e a constante catalítica (Kcat) encontrada foi 1,364 . 10-³.s-³. São relatados na literatura poucos compostos químicos capazes de inibir a atividade catalítica da PDI. Assim, para verificar se compostos radicalares estáveis desempenham essa atividade, foram testados nitróxidos piperidínicos como possíveis inibidores de PDI. Esses compostos, que possuem propriedades antioxidantes, antiinflamatórias e radioprotetoras, apresentam efeito “scavenger” sobre diferentes espécies radicalares, dentre as quais, radicais tiila. O nitróxido 4-hidroxi-2,2,6,6- tetrametilpiperidina-1-oxil (Tempol) mostrou-se um inibidor pouco potente da atividade redutase da enzima. Entretanto, três outros nitróxidos, sintetizados especificamente para este trabalho, demonstraram maior poder de inibição, com uma correlação direta com o aumento de hidrofobicidade das estruturas químicas dos mesmos. Essa capacidade de inibição foi confirmada sobre a atividade de PDI presente em plaquetas humanas, corroborando a hipótese de que os nitróxidos são candidatos a novos fármacos moduladores de funções celulares onde esteja envolvida a atividade de PDI.application/pdfporUniversidade Federal de AlfenasPrograma de Pós-Graduação em QuímicaUNIFAL-MGBrasilInstituto de Químicainfo:eu-repo/semantics/openAccesshttp://creativecommons.org/licenses/by-nc-nd/4.0/Cinética de enzimasChaperonas MolecularesInibidores EnzimáticasFISICO-QUIMICA::CINETICA QUIMICA E CATALISEEstudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalíticainfo:eu-repo/semantics/masterThesisinfo:eu-repo/semantics/publishedVersion13282530788267823066006005507836868851247592reponame:Repositório Institucional da Universidade Federal de Alfenas - RiUnifalinstname:Universidade Federal de Alfenas (UNIFAL)instacron:UNIFALOliveira, Altamir Fernandes DeLICENSElicense.txtlicense.txttext/plain; charset=utf-81987https://repositorio.unifal-mg.edu.br/bitstreams/30a7352f-75d6-49b8-973a-f0aa8163c22d/download31555718c4fc75849dd08f27935d4f6bMD51CC-LICENSElicense_urllicense_urltext/plain; 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dc.title.pt-BR.fl_str_mv Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
title Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
spellingShingle Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
Oliveira, Altamir Fernandes De
Cinética de enzimas
Chaperonas Moleculares
Inibidores Enzimáticas
FISICO-QUIMICA::CINETICA QUIMICA E CATALISE
title_short Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
title_full Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
title_fullStr Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
title_full_unstemmed Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
title_sort Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica
author Oliveira, Altamir Fernandes De
author_facet Oliveira, Altamir Fernandes De
author_role author
dc.contributor.author.fl_str_mv Oliveira, Altamir Fernandes De
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/0963588859777460
dc.contributor.referee1.fl_str_mv D'Assunção, Lázaro Moscardini
dc.contributor.referee2.fl_str_mv Florenzano, Fábio Herbst
dc.contributor.advisor1.fl_str_mv Brigagão, Maísa Ribeiro Pereira Lima
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/2974319270935111
contributor_str_mv D'Assunção, Lázaro Moscardini
Florenzano, Fábio Herbst
Brigagão, Maísa Ribeiro Pereira Lima
dc.subject.por.fl_str_mv Cinética de enzimas
Chaperonas Moleculares
Inibidores Enzimáticas
topic Cinética de enzimas
Chaperonas Moleculares
Inibidores Enzimáticas
FISICO-QUIMICA::CINETICA QUIMICA E CATALISE
dc.subject.cnpq.fl_str_mv FISICO-QUIMICA::CINETICA QUIMICA E CATALISE
description Protein disulfide isomerase (PDI, EC 5.3.4.1) belonging to the thioredoxin superfamily, is a thiol oxidoreductase that catalyzes the oxidation and reduction of thiols and intramolecular disulfide isomerization. This chaperone, such activity is dependent of cysteine located on the active sites, is present in the endoplasmic reticulum (ER) and / or plasma membrane of eukaryotic cells. Previous studies of the catalytic activity of PDI were performed using different pseudo-substrates, among them, the di-eosin-glutathione disulfide (Di-E-GSSG), described as a usefull tool for monitoring the disulfide reductase activity of PDI . In this work, the synthesis and chromatographic purification of Di-E-GSSG were performed and the purity of the probe was verified by high performance liquid chromatography (HPLC). The enzyme kinetics of the reductase activity of recombinant PDI isolated over Di-E-GSSG was studied, characterizing the main physicochemical parameters of the enzyme through the formation of the fluorescent monomer (λexc=521nm; λemi=542nm) eosin-reduced glutathione (E-GSH). The value of the Michaelis-Menten constant (Km) was found to be 520.5 ± 129.8 nM, the maximum velocity of catalysis (Vmáx) was determined as 1,637 ± 0.1526 nM.min-¹ and the catalytic constant (Kcat) found was 1.364 . 10-³.s-¹. Few chemical compounds able to inhibit catalytic activity of PDI were reported. Thus, to verify if stable free radical compounds display this activity were tested piperidine nitroxides as potential inhibitors of PDI. These compounds, which have antioxidant, anti-inflammatory and radioprotective properties are “scavengers” of different radical species, among them, thyil radicals. The nitroxide 4-hydroxy-2,2,6,6-tetrametilpiperidine-1-oxyl (Tempol) was a weak inhibitor of PDI reductase activity. However, three other nitroxides specifically synthesized for this study showed higher inhibition power, with a direct correlation between increasing the hydrophobicity of the chemical structures and inhibitory action. This ability was confirmed by assays with PDI found in human platelets, confirming the hypothesis that the nitroxides are candidates for new drugs to modulate cellular functions involving the PDI activity.
publishDate 2010
dc.date.issued.fl_str_mv 2010-12-07
dc.date.accessioned.fl_str_mv 2015-11-18T17:06:52Z
dc.type.driver.fl_str_mv info:eu-repo/semantics/masterThesis
dc.type.status.fl_str_mv info:eu-repo/semantics/publishedVersion
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dc.identifier.citation.fl_str_mv OLIVEIRA, Altamir Fernandes de. Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica. 2010. 93 f. Dissertação (Mestrado em Química) - Universidade Federal de Alfenas, Alfenas, MG, 2010.
dc.identifier.uri.fl_str_mv https://repositorio.unifal-mg.edu.br/handle/123456789/723
identifier_str_mv OLIVEIRA, Altamir Fernandes de. Estudo cinético da proteína dissulfeto isomerase: nitróxidos como reguladores da atividade catalítica. 2010. 93 f. Dissertação (Mestrado em Química) - Universidade Federal de Alfenas, Alfenas, MG, 2010.
url https://repositorio.unifal-mg.edu.br/handle/123456789/723
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dc.publisher.country.fl_str_mv Brasil
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