Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi

Detalhes bibliográficos
Ano de defesa: 2011
Autor(a) principal: Viviane Grazielle da Silva
Orientador(a): Não Informado pela instituição
Banca de defesa: Não Informado pela instituição
Tipo de documento: Dissertação
Tipo de acesso: Acesso aberto
Idioma: por
Instituição de defesa: Universidade Federal de Minas Gerais
Programa de Pós-Graduação: Não Informado pela instituição
Departamento: Não Informado pela instituição
País: Não Informado pela instituição
Palavras-chave em Português:
Bioquímica e imunologia
Trypanosoma cruzi
Doença de Chagas
Reparo de Erro de Pareamento de DNA
Doença de chagas
MMR
DNA
Link de acesso: https://hdl.handle.net/1843/42837
Resumo: Trypanosoma cruzi, etiologic agent of Chagas disease, presents a highly heterogeneous population structure, characterized by the occurrence of different strains with different biochemical and morphological characteristics. This complex population structure may be correlated with different clinical manifestations of disease, parasite's ability to infect different hostages and geographical distribution presented by the strains. Intra-specific variability can be a result of a balance between genomic stability and generation of genetic variability. Several mechanisms can be involved in maintaining this balance, for example, DNA mismatch repair – MMR. Initial studies on the MMR in T. cruzi led to the discovery that MSH2 - the main protein of the MMR - exists in three isoforms in the parasite, named TcMSH2 A, B and C, according to Tcmsh2 data sequences present in the genome of different strains. Experimental evidence indicates that strains presenting the isoform TcMSH2 A have a more efficient MMR when compared to strains that have TcMSH2 B and/or C isoforms. These observations led us to speculate that differences in MMR activity could account for a lower genetic variability found in strains belonging to MSH2-A haplogroup. In order to investigate the role of the MSH2 protein, we tried to obtain knockout parasites for this gene. Single knockouts parasites are more susceptible to hydrogen peroxide treatment and accumulate more 8-oxoguanine in mitochondrial DNA than wild type parasites, despite the fact that there are no differences after treatment with mutagenic agents. With the aim to better investigate the role of MSH2 in response to oxidative stress, in the present work we investigated MSH2 cellular localization. Antibodies raised against a recombinant form of MSH2 produced in mice were used in immunolocalization and western blot assays. Those experiments have shown that the serum produced in mice is able to recognize the native protein in two different molecular weight proteins, with different subcellular localization. Based on that, we have speculated that the lower molecular weight protein, which is localized at extract fraction correspondent to the cytoplasm, could be involved in mitochondrial DNA repair. Simultaneously, to investigate if TcMSH2 role in response to oxidative damage is dependent of other MMR proteins, we began to characterize them. Two different strategies were used to knockout Tcmsh6. And we also tried to elucidate TcMSH6 subcellular localization after its over-expression in fusion with RFP.
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spelling Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruziBioquímica e imunologiaTrypanosoma cruziDoença de ChagasReparo de Erro de Pareamento de DNATrypanosoma cruziDoença de chagasMMRDNATrypanosoma cruzi, etiologic agent of Chagas disease, presents a highly heterogeneous population structure, characterized by the occurrence of different strains with different biochemical and morphological characteristics. This complex population structure may be correlated with different clinical manifestations of disease, parasite's ability to infect different hostages and geographical distribution presented by the strains. Intra-specific variability can be a result of a balance between genomic stability and generation of genetic variability. Several mechanisms can be involved in maintaining this balance, for example, DNA mismatch repair – MMR. Initial studies on the MMR in T. cruzi led to the discovery that MSH2 - the main protein of the MMR - exists in three isoforms in the parasite, named TcMSH2 A, B and C, according to Tcmsh2 data sequences present in the genome of different strains. Experimental evidence indicates that strains presenting the isoform TcMSH2 A have a more efficient MMR when compared to strains that have TcMSH2 B and/or C isoforms. These observations led us to speculate that differences in MMR activity could account for a lower genetic variability found in strains belonging to MSH2-A haplogroup. In order to investigate the role of the MSH2 protein, we tried to obtain knockout parasites for this gene. Single knockouts parasites are more susceptible to hydrogen peroxide treatment and accumulate more 8-oxoguanine in mitochondrial DNA than wild type parasites, despite the fact that there are no differences after treatment with mutagenic agents. With the aim to better investigate the role of MSH2 in response to oxidative stress, in the present work we investigated MSH2 cellular localization. Antibodies raised against a recombinant form of MSH2 produced in mice were used in immunolocalization and western blot assays. Those experiments have shown that the serum produced in mice is able to recognize the native protein in two different molecular weight proteins, with different subcellular localization. Based on that, we have speculated that the lower molecular weight protein, which is localized at extract fraction correspondent to the cytoplasm, could be involved in mitochondrial DNA repair. Simultaneously, to investigate if TcMSH2 role in response to oxidative damage is dependent of other MMR proteins, we began to characterize them. Two different strategies were used to knockout Tcmsh6. And we also tried to elucidate TcMSH6 subcellular localization after its over-expression in fusion with RFP.Universidade Federal de Minas Gerais2022-07-01T12:54:03Z2025-09-09T00:08:39Z2022-07-01T12:54:03Z2011-02-07info:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesisapplication/pdfhttps://hdl.handle.net/1843/42837porViviane Grazielle da Silvainfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UFMGinstname:Universidade Federal de Minas Gerais (UFMG)instacron:UFMG2025-09-09T00:08:39Zoai:repositorio.ufmg.br:1843/42837Repositório InstitucionalPUBhttps://repositorio.ufmg.br/oairepositorio@ufmg.bropendoar:2025-09-09T00:08:39Repositório Institucional da UFMG - Universidade Federal de Minas Gerais (UFMG)false
dc.title.none.fl_str_mv Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
title Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
spellingShingle Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
Viviane Grazielle da Silva
Bioquímica e imunologia
Trypanosoma cruzi
Doença de Chagas
Reparo de Erro de Pareamento de DNA
Trypanosoma cruzi
Doença de chagas
MMR
DNA
title_short Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
title_full Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
title_fullStr Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
title_full_unstemmed Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
title_sort Estudo do papel das proteínas MSH2 e MSH6 na resposta a danos no DNA em Trypanosoma cruzi
author Viviane Grazielle da Silva
author_facet Viviane Grazielle da Silva
author_role author
dc.contributor.author.fl_str_mv Viviane Grazielle da Silva
dc.subject.por.fl_str_mv Bioquímica e imunologia
Trypanosoma cruzi
Doença de Chagas
Reparo de Erro de Pareamento de DNA
Trypanosoma cruzi
Doença de chagas
MMR
DNA
topic Bioquímica e imunologia
Trypanosoma cruzi
Doença de Chagas
Reparo de Erro de Pareamento de DNA
Trypanosoma cruzi
Doença de chagas
MMR
DNA
description Trypanosoma cruzi, etiologic agent of Chagas disease, presents a highly heterogeneous population structure, characterized by the occurrence of different strains with different biochemical and morphological characteristics. This complex population structure may be correlated with different clinical manifestations of disease, parasite's ability to infect different hostages and geographical distribution presented by the strains. Intra-specific variability can be a result of a balance between genomic stability and generation of genetic variability. Several mechanisms can be involved in maintaining this balance, for example, DNA mismatch repair – MMR. Initial studies on the MMR in T. cruzi led to the discovery that MSH2 - the main protein of the MMR - exists in three isoforms in the parasite, named TcMSH2 A, B and C, according to Tcmsh2 data sequences present in the genome of different strains. Experimental evidence indicates that strains presenting the isoform TcMSH2 A have a more efficient MMR when compared to strains that have TcMSH2 B and/or C isoforms. These observations led us to speculate that differences in MMR activity could account for a lower genetic variability found in strains belonging to MSH2-A haplogroup. In order to investigate the role of the MSH2 protein, we tried to obtain knockout parasites for this gene. Single knockouts parasites are more susceptible to hydrogen peroxide treatment and accumulate more 8-oxoguanine in mitochondrial DNA than wild type parasites, despite the fact that there are no differences after treatment with mutagenic agents. With the aim to better investigate the role of MSH2 in response to oxidative stress, in the present work we investigated MSH2 cellular localization. Antibodies raised against a recombinant form of MSH2 produced in mice were used in immunolocalization and western blot assays. Those experiments have shown that the serum produced in mice is able to recognize the native protein in two different molecular weight proteins, with different subcellular localization. Based on that, we have speculated that the lower molecular weight protein, which is localized at extract fraction correspondent to the cytoplasm, could be involved in mitochondrial DNA repair. Simultaneously, to investigate if TcMSH2 role in response to oxidative damage is dependent of other MMR proteins, we began to characterize them. Two different strategies were used to knockout Tcmsh6. And we also tried to elucidate TcMSH6 subcellular localization after its over-expression in fusion with RFP.
publishDate 2011
dc.date.none.fl_str_mv 2011-02-07
2022-07-01T12:54:03Z
2022-07-01T12:54:03Z
2025-09-09T00:08:39Z
dc.type.status.fl_str_mv info:eu-repo/semantics/publishedVersion
dc.type.driver.fl_str_mv info:eu-repo/semantics/masterThesis
format masterThesis
status_str publishedVersion
dc.identifier.uri.fl_str_mv https://hdl.handle.net/1843/42837
url https://hdl.handle.net/1843/42837
dc.language.iso.fl_str_mv por
language por
dc.rights.driver.fl_str_mv info:eu-repo/semantics/openAccess
eu_rights_str_mv openAccess
dc.format.none.fl_str_mv application/pdf
dc.publisher.none.fl_str_mv Universidade Federal de Minas Gerais
publisher.none.fl_str_mv Universidade Federal de Minas Gerais
dc.source.none.fl_str_mv reponame:Repositório Institucional da UFMG
instname:Universidade Federal de Minas Gerais (UFMG)
instacron:UFMG
instname_str Universidade Federal de Minas Gerais (UFMG)
instacron_str UFMG
institution UFMG
reponame_str Repositório Institucional da UFMG
collection Repositório Institucional da UFMG
repository.name.fl_str_mv Repositório Institucional da UFMG - Universidade Federal de Minas Gerais (UFMG)
repository.mail.fl_str_mv repositorio@ufmg.br
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