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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
1

Regeneration of gingival tissue using in situ tissue engineering with collagen scaffold / 生体内再生の手法によるコラーゲン足場を用いた歯肉組織の再生

Hatayama, Takahide 23 July 2019 (has links)
京都大学 / 0048 / 新制・論文博士 / 博士(医学) / 乙第13265号 / 論医博第2179号 / 新制||医||1038(附属図書館) / (主査)教授 別所 和久, 教授 安達 泰治, 教授 戸口田 淳也 / 学位規則第4条第2項該当 / Doctor of Medical Science / Kyoto University / DFAM
2

Lokalisation av cathepsin B och cystatin C i gingival vävnad från patienter med kronisk parodontit

Svensson, Eva-Liisa, Thulin, Regina January 2012 (has links)
Cysteinproteaset cathepsin B har en trolig roll i vävnadsnedbrytningen vid kronisk parodontit då det visats kunna bryta ner extracellulära komponenter. Cystatin C är en fysiologisk inhibitor av cathepsin B och båda har kopplats till parodontal sjukdom. Syftet med studien var att undersöka närvaro av samt lokalisera cathepsin B och cystatin C i gingivala biopsier från patienter med kronisk parodontit. Närvaro och lokalisation av cathepsin Bs och cystatin Cs demonstrerades genom immunohistokemisk metod av kryostatsnittad vävnad. Polyklonal kanin anti-human primär antikropp för både enzym och inhibitor användes. För identifiering av primära antikroppar användes Dako REAL™ EnVision™ Detection System. Granskning skedde i ljusmikroskop. Studien visar på en närvaro av både enzym och inhibitor i epitel och bindväv i parodontalt sjuk vävnad. Cathepsin B lokaliserades i stor utsträckning till bindväven, främst perivaskulärt. I epitelet lokaliserades endast ett fåtal infärgade celler. Cystatin C hade i bindväven en diffus utbredning vilket gjorde lokalisation till specifika cellpopulationer svår. I epitelet sågs en tydlig infärgning kring/i celler med dendritiskt utseende. Dessa celler identifierades som sannolika langerhanska celler. / The cysteine protease cathepsin B has been shown to have a possible role in tissue destruction in chronic periodontitis, as it has been shown to degrade extracellular components. Cystatin C is a physiological inhibitor of cathepsin B and both are associated with periodontal disease. The aim with this study was to investigate the presence and localization of cathepsin B and cystatin C in gingival biopsies from patients with chronic periodontitis. Cathepsin B's and cystatin C’s presence and localization was demonstrated by immunohistochemical method of cryostat sectioned tissue from patients with chronic periodontitis. Polyclonal rabbit anti-human primary antibody for both the enzyme and the inhibitor were used. Identification of the primary antibodies were confirmed with Dako REAL ™ EnVision ™ Detection System. The sectioned tissue was analysed by using light microscopy. Our study indicates a presence of both enzyme and inhibitor in epithelial and connective tissue from patients with periodontal disease. Cathepsin B was localized mainly to the connective tissue, primarily to the perivascular space. In the epithelium only a few stained cells were identified. In the connective tissue, cystatin C had a diffuse distribution. Therefor it was difficult to distinguish the specific cell populations associated with the inhibitor. The epithelium showed a clear staining around/in dendritic cells. These cells were identified as probable Langerhans cells.
3

Estudo da expressão e produção de componentes do sistema renina-angiotensina por fibroblastos de gengiva e ligamento periodontal humanos / Study of expression and production of the renin-angiotensin system components by gingival and periodontal ligament human fibroblasts

Ishikiriama, Bella Luna Colombini 13 April 2012 (has links)
O Sistema Renina-angiotensina (SRA), e um sistema capaz de gerar hormonios peptideos com grande impacto na regulacao cardiovascular e na patogenese das doencas cardiovasculares. Este sistema opera, por meio das acoes da Angiotensina II, tanto em nivel sistemico (endocrino) quanto tecidual (local, paracrino/autocrino) controlando importantes funcoes, varias delas relacionadas a facilitacao da instalacao e progressao do processo inflamatorio. Por este motivo, a producao desta proteina nos tecidos pode estar relacionada a patogenese de muitas doencas, dentre elas a doenca periodontal (DP), tendo em vista seu carater infeccioso-inflamatorio e os achados da literatura que mostram que a inibicao da formacao de Ang II, diminui a perda óssea da DP em animais. Desta forma, o presente trabalho teve como objetivos: Avaliar in vitro, a) A expressao de componentes do SRA (ANGT, RENINA, ECA, ECA-2, AT1, AT2 e Mas) por fibroblastos de gengiva e ligamento periodontal humanos, por RT-qPCR; b) A producao de componentes do SRA (RENINA, ECA, ECA-2) no sobrenadante de culturas de fibroblastos de gengiva e ligamento periodontal humanos, por ELISA; c) A producao dos receptores do SRA (AT1, AT2 e Mas), nestes fibroblastos, por Imunofluorescencia e d) Se a expressao e a producao dos componentes do SRA por fibroblastos de gengiva e ligamento periodontal humanos, se alteram com a estimulacao por LPS de P. gingivalis e E. coli. Apos a coleta, os dados foram analisados com o auxilio do programa GraphPad Prism 5.0. por meio da analise de variancia a 2 criterios (ANOVA-two way) seguida do pos teste de Bonferroni, com nivel de significancia de 5% para a verificacao das possíveis diferencas. Foi detectada a expressao genica para alguns dos componentes do SRA (ANGT, RENINA, ECA, AT1) por fibroblastos tanto de gengiva quanto de ligamento periodontal. Foi detectada ainda uma expressao genica diferenciada entre fibroblastos de gengiva e ligamento periodontal para a ECA, sendo significativamente maior nos fibroblastos da gengiva. Houve imunomarcacao positiva tanto nos fibroblastos de gengiva quanto de ligamento periodontal compativel com a presenca dos receptores AT1 e Mas. Pode-se observar por fim que o contato com LPS de P. gingivalis e E. coli, na concentracao de 10 g/mL/24 h, nao alteram a expressão dos componentes do SRA. Portanto, pode-se concluir que os fibroblastos tanto de gengiva quanto de ligamento periodontal apesar de nao expressarem e produzirem todos oscomponentes do SRA necessarios para a formacao local de Ang II, poderiam contribuir, ainda que parcialmente, com outras celulas do microambiente dos tecidos periodontais para a formacao e acao locais da Ang II, e assim, para a instalacao e progressao da DP. / The Renin-angiotensin system (RAS) can generate hormones that have a high-impact on cardiovascular regulation as well as in the pathogenesis of cardiovascular disease. This system acts through both systemic (endocrine) and local (paracrine/autocrine) effects of Angiotensin II, controlling important functions related to the facilitation of installation and progression of the inflammatory process. For this reason, this proteins production in tissues can be associated to the pathogenesis of many diseases, including periodontal disease (PD). In the PD setting, a infectious-inflammatory characterized disease, the literature findings shows that inhibition of the Ang II formation can decrease the bone loss in animals. In this context, the aims of the present study were: to investigate in vitro: a) the expression of RAS components (ANGT, RENIN, ECA, ECA- 2, AT1, AT2 and Mas) by human gingival and periodontal ligament fibroblasts by RT-qPCR; b) the production of RAS receptors (AT1, AT2 and Mas) by human cultured gingival and periodontal ligament fibroblasts by Immunofluorescence and d) the production of RAS components (RENIN, ECA, ECA-2) if the expression and production of RAS components by gingival and periodontal ligament fibroblasts modify under P. gingivalis and E. coli LPS stimulation. After collected, the data were analysed using GraphPad Prism 5.0, by the two way ANOVA followed by Bonferroni post test with a significance level of 5%. Gene expression was detected for some of the RAS components (ANGT, RENIN, ECA, AT1) by both gingival and periodontal ligament fibroblasts. It was detected a differential gene expression between gingival and periodontal ligament fibroblasts for ECA, being significantly higher in gingival fibroblasts. There was a stain in Immunofluorescence compatible with the production of RAS receptors (AT1 and Mas). It must be noted that the stimulation with P. gingivalis and E. coli LPS, in a concentration of 10 g/mL/24 h, did not altered the expression of RAS components. In conclusion, despite of neither gingival or periodontal ligament fibroblasts express all components of RAS, needed to local formation of Ang II, they might also contribute to the local formation and action of Ang II and in consequence, to the installation and the progression of DP.
4

Estudo da expressão e produção de componentes do sistema renina-angiotensina por fibroblastos de gengiva e ligamento periodontal humanos / Study of expression and production of the renin-angiotensin system components by gingival and periodontal ligament human fibroblasts

Bella Luna Colombini Ishikiriama 13 April 2012 (has links)
O Sistema Renina-angiotensina (SRA), e um sistema capaz de gerar hormonios peptideos com grande impacto na regulacao cardiovascular e na patogenese das doencas cardiovasculares. Este sistema opera, por meio das acoes da Angiotensina II, tanto em nivel sistemico (endocrino) quanto tecidual (local, paracrino/autocrino) controlando importantes funcoes, varias delas relacionadas a facilitacao da instalacao e progressao do processo inflamatorio. Por este motivo, a producao desta proteina nos tecidos pode estar relacionada a patogenese de muitas doencas, dentre elas a doenca periodontal (DP), tendo em vista seu carater infeccioso-inflamatorio e os achados da literatura que mostram que a inibicao da formacao de Ang II, diminui a perda óssea da DP em animais. Desta forma, o presente trabalho teve como objetivos: Avaliar in vitro, a) A expressao de componentes do SRA (ANGT, RENINA, ECA, ECA-2, AT1, AT2 e Mas) por fibroblastos de gengiva e ligamento periodontal humanos, por RT-qPCR; b) A producao de componentes do SRA (RENINA, ECA, ECA-2) no sobrenadante de culturas de fibroblastos de gengiva e ligamento periodontal humanos, por ELISA; c) A producao dos receptores do SRA (AT1, AT2 e Mas), nestes fibroblastos, por Imunofluorescencia e d) Se a expressao e a producao dos componentes do SRA por fibroblastos de gengiva e ligamento periodontal humanos, se alteram com a estimulacao por LPS de P. gingivalis e E. coli. Apos a coleta, os dados foram analisados com o auxilio do programa GraphPad Prism 5.0. por meio da analise de variancia a 2 criterios (ANOVA-two way) seguida do pos teste de Bonferroni, com nivel de significancia de 5% para a verificacao das possíveis diferencas. Foi detectada a expressao genica para alguns dos componentes do SRA (ANGT, RENINA, ECA, AT1) por fibroblastos tanto de gengiva quanto de ligamento periodontal. Foi detectada ainda uma expressao genica diferenciada entre fibroblastos de gengiva e ligamento periodontal para a ECA, sendo significativamente maior nos fibroblastos da gengiva. Houve imunomarcacao positiva tanto nos fibroblastos de gengiva quanto de ligamento periodontal compativel com a presenca dos receptores AT1 e Mas. Pode-se observar por fim que o contato com LPS de P. gingivalis e E. coli, na concentracao de 10 g/mL/24 h, nao alteram a expressão dos componentes do SRA. Portanto, pode-se concluir que os fibroblastos tanto de gengiva quanto de ligamento periodontal apesar de nao expressarem e produzirem todos oscomponentes do SRA necessarios para a formacao local de Ang II, poderiam contribuir, ainda que parcialmente, com outras celulas do microambiente dos tecidos periodontais para a formacao e acao locais da Ang II, e assim, para a instalacao e progressao da DP. / The Renin-angiotensin system (RAS) can generate hormones that have a high-impact on cardiovascular regulation as well as in the pathogenesis of cardiovascular disease. This system acts through both systemic (endocrine) and local (paracrine/autocrine) effects of Angiotensin II, controlling important functions related to the facilitation of installation and progression of the inflammatory process. For this reason, this proteins production in tissues can be associated to the pathogenesis of many diseases, including periodontal disease (PD). In the PD setting, a infectious-inflammatory characterized disease, the literature findings shows that inhibition of the Ang II formation can decrease the bone loss in animals. In this context, the aims of the present study were: to investigate in vitro: a) the expression of RAS components (ANGT, RENIN, ECA, ECA- 2, AT1, AT2 and Mas) by human gingival and periodontal ligament fibroblasts by RT-qPCR; b) the production of RAS receptors (AT1, AT2 and Mas) by human cultured gingival and periodontal ligament fibroblasts by Immunofluorescence and d) the production of RAS components (RENIN, ECA, ECA-2) if the expression and production of RAS components by gingival and periodontal ligament fibroblasts modify under P. gingivalis and E. coli LPS stimulation. After collected, the data were analysed using GraphPad Prism 5.0, by the two way ANOVA followed by Bonferroni post test with a significance level of 5%. Gene expression was detected for some of the RAS components (ANGT, RENIN, ECA, AT1) by both gingival and periodontal ligament fibroblasts. It was detected a differential gene expression between gingival and periodontal ligament fibroblasts for ECA, being significantly higher in gingival fibroblasts. There was a stain in Immunofluorescence compatible with the production of RAS receptors (AT1 and Mas). It must be noted that the stimulation with P. gingivalis and E. coli LPS, in a concentration of 10 g/mL/24 h, did not altered the expression of RAS components. In conclusion, despite of neither gingival or periodontal ligament fibroblasts express all components of RAS, needed to local formation of Ang II, they might also contribute to the local formation and action of Ang II and in consequence, to the installation and the progression of DP.

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