Global ETD Search

141	A influência da pinealectomia na funcionalidade das células beta pancreáticas. / The influence of pinealectomy in pancreatic beta cell functionality. Daniel Simões de Jesus 01 August 2011 (has links) As ilhotas pancreáticas têm em sua constituição as células <font face=\"Symbol\">b pancreáticas, as quais têm como função secretar insulina. A melatonina é secretada pela glândula pineal. No entanto, a ausência da melatonina, por meio da pinealectomia (PINX), induz diversas alterações nas funções celulares. A NAD(P)H oxidase é responsável pela produção de ânions superóxido. Nosso estudo teve como objetivo avaliar uma possível modulação da NAD(P)H oxidase pela PINX no Zeitgeber Time 6 e 18. Os resultados demonstram que a PINX induz alterações na funcionalidade das ilhotas pancreáticas, alterando a secreção de insulina estimulada pela glicose, o metabolismo da glicose, e o conteúdo de espécies reativas de oxigênio (EROs). Entretanto, não induz alterações nos respectivos ZTs na expressão protéica das subunidades p22phox, p47phox e gp91phox. Demonstramos que a pinealectomia induz alteração no padrão rítmico metabólico e secretório nas ilhotas isoladas, tendo a NAD(P)H oxidase uma possível participação no desenvolvimento nas alterações observadas. / Pancreatic islets are constituted by pancreatic cells, which main function is to secrete insulin. Melatonin is secreted by the pineal gland. However, the absence of melatonin by pinealectomy (PINX) induces several changes in cellular functions. The NAD(P)H oxidase is responsible for producing superoxide. Our study aimed to evaluate the possible modulation of NAD(P)H oxidase by pinealectomy in Zeitgeber Time 6:18. Our results show that the absence of melatonin induced by pinealectomy induces changes in the functionality of pancreatic islets, such as the insulin secretion stimulated by glucose, the glucose metabolism, and the content of reactive oxygen species (ROS). However, it does not induce changes in their respective Zts in the protein expression of the subunits p22phox, p47phox and gp91phox. We demonstrated that pinealectomy induces changes in metabolic and secretory rhythm pattern in isolated islets, being the NAD(P)H oxidase a possibly responsible for the changes observed. Ativação enzimática Glândula pineal Ilhotas de Langerhans Insulina Melatonina Secreção Enzyme activation Insulin Islets of Langerhans Melatonin Pineal gland Secretion
142	Mécanismes moléculaires et cellulaires dans l’induction des réponses T helper folliculaires après vaccination cutanée / Molecular and cellular mecanisms in the induction of T follicular helper responses after cutaneous vaccination Levin, Clément 12 December 2016 (has links) La vaccination du tissu cutané présente un fort potentiel, car elle permet le ciblage de l’antigène aux populations de cellules dendritiques uniques et spécialisées de la peau, et le recrutement de cellules inflammatoires du sang.Les cellules T helper folliculaires (TFH) jouent un rôle crucial dans l’établissement de la réponse humorale. Cependant, les interactions cellulaires et moléculaires qui gouvernent leur induction dans un contexte de vaccination restent à élucider.Mon projet de thèse a eu pour but de mieux comprendre les mécanismes d’induction des réponses TFH et humorales, par l’étude des événements précoces ayant lieu aux sites d’immunisation et d’induction de l’immunité adaptative après vaccination cutanée. L’utilisation de modèles murins nous a permis d’évaluer la contribution de différentes populations de la peau, du ganglion, et du sang dans la mise en place de ces réponses après immunisation intradermique avec un antigène particulaire présentant l’antigène modèle p24 du VIH. Cette étude a révélé un rôle crucial des cellules de Langerhans et des cellules dendritiques migratoires de la peau dans l’induction de réponses TFH et humorales.Nous avons ensuite évalué la capacité de différentes formulations d’adjuvants à polariser la réponse TFH et humorale contre un antigène de l’enveloppe du VIH à fort potentiel vaccinal. L’utilisation de l’émulsion IFA favorise l’induction des cellules TFH et induit la production d’anticorps neutralisants des souches du VIH.Ces résultats soulignent l’importance de cibler les DCs de la peau par l’utilisation de voies de vaccination pertinentes et l’utilisation d’adjuvants capables de favoriser la réponse cellulaire TFH. / Skin vaccination is of great interest, as it enables targeting of the antigen to unique and specialized dendritic cell populations of the skin, as well as recruitment of inflammatory blood cells.T follicular helper (TFH) cells play a critical role in the setting of the humoral response. However, the cellular and molecular interactions that underlie their induction after vaccination remain unknown.My thesis project aimed at understanding the immune mechanisms by which skin vaccination could favor the induction of TFH and humoral immune responses by studying the early events that take place in tissue and lymph node.Using mice models, we evaluated the relative contributions of various populations from the skin, lymph node and blood in the setting of TFH cell responses after intradermal immunization with nanoparticles coated with p24 antigen from HIV. This revealed a crucial role of Langerhans cells and skin migratory dendritic cells in the induction of TFH and germinal center responses.We then evaluated the ability of different adjuvant formulations to polarize the TFH and humoral response against a promising vaccine antigen from HIV envelope protein. Emulsifying the antigen in IFA favors the induction of TFH cells and induces the production of neutralizing antibodies able to block viral infection.This work highlights the relevance of targeting skin dendritic cells by using relevant vaccination routes and adjuvant formulation able to induce TFH cell responses. Vaccination cutanée Cellule T helper folliculaire Cellule de Langerhans Nanoparticule VIH Inflammation Skin vaccination T follicular helper cell Langerhans cell 571.96
143	Transcription factors and downstream genes modulating TNF-gas + IFN-gcs induced beta cell apoptosis Barthson, Jenny 08 April 2013 (has links) In type 1 diabetes (T1D) a combination of genetic predisposition and environmental factors triggers islet inflammation (insulitis) leading to a selective and gradual destruction of the pancreatic beta cells. Beta cells mainly die through apoptosis, triggered at least in part by pro-inflammatory cytokines such as IL-1β, TNF-α and IFN-γ. Recent findings suggest that the mitochondrial pathway of cell death is involved in this death cascade. Array analysis indicated that TNF-α+IFN-γ induces transcription factors such as NF-ĸB, STAT1, and AP-1 in beta cells. We presently aimed to examine the pathway(s) of apoptosis triggered by TNF-α+IFN-γ in beta cells. <p>TNF-α+IFN-γ induces beta cell apoptosis through the intrinsic pathway of cell death. This involved activation of the BH3 only proteins DP5, PUMA and Bim. Knockdown (KD) of either DP5 or PUMA or both led to a partial protection of INS-1E cells (12-20%), while silencing Bim led to about 60% protection against cytokine-induced apoptosis. Bim is transcriptionally induced by activated STAT1. TNF-α+IFN-γ also induces downregulation of Bcl-XL, an anti-apoptotic Bcl-2 gene which inhibits Bim. Knocking down Bcl-XL alone led to increase in apoptosis, but this was prevented by the parallel KD of Bim.<p>The ultimate goal of our research is to protect beta cells from the autoimmune assault. Previous data revealed that JunB inhibits ER stress and apoptosis in beta cells treated with IL-β+IFN-γ. Here, TNF-α+IFN-γ up-regulated the expression of JunB which was downstream of activated NF-ĸB. JunB KD exacerbated TNF-α+IFN-γ induced beta cell death in primary rat beta cells and INS-1E cells. The gene networks affected by JunB were studied by microarray analysis. JunB regulates 20-25% of the cytokine-modified beta cell genes, including the transcription factor ATF3 and Bcl-XL. ATF3 expression was increased in cytokine-treated human islets and in vitro silencing of JunB led to >60% reduction in ATF3 overexpression. We confirmed direct JunB regulation of the ATF3 promoter by its binding to an ATF/CRE site. Silencing of ATF3 aggravated TNF-α+IFN-γ induced cell death in beta cells and led to the downregulation of Bcl-XL expression in INS-1E cells. Pharmacological upregulation of JunB using forskolin led to upregulation of ATF3 and consistent protection of these cells against cytokine-induced cell death, while genetic overexpression of JunB in mice increased ATF3 expression in the pancreatic islets and reversed the pro-apoptotic effects of cytokines on beta cells (±40 % protection). <p>As a whole, our findings indicate that TNF-α+IFN-γ triggers beta cell apoptosis by the upregulation of the pro-apoptotic protein Bim and downregulation of the Bcl-XL protein. These deleterious effects are at least in part antagonized by JunB via activation of ATF3. <p><p>Dans le diabète de type 1 (DT1), la combinaison de facteurs génétiques de prédisposition et de l'environnement déclenche l'inflammation des îlots de Langerhans (insulite) conduisant à une destruction sélective et progressive des cellules bêta du pancréas. Les cellules bêta meurent principalement d’apoptose, déclenchée au moins en partie par les cytokines pro-inflammatoires sécrétées par les cellules immunitaires comme l’IL-β, le TNF-α l’IFN-γ. De récentes découvertes suggèrent que la voie mitochondriale de la mort cellulaire jouerait un rôle dans la mort de ces cellules. L'analyse de réseaux de gène utilisant les biopuces d’ADN indique que l’association TNF-α+IFN-γ induit l’activation de facteurs de transcription tels que NF-ĸB, STAT1 et AP-1 dans la cellule bêta. Dans ce contexte, nous avons cherché à examiner les voies de l'apoptose déclenchées par le TNF-α+IFN-γ dans la cellule bêta. <p>En présence de TNF-α+IFN-γ les cellules bêta meurent par apoptose via la voie intrinsèque. L’activation des protéines pro-apoptotiques « BH3-seulement » dont DP5, PUMA et Bim étaient en cause de cette apoptose. Le « knockdown »1 (KD), de DP5 ou de PUMA, ou des deux en même temps conduit à une protection partielle des cellules INS-1E (12-20%), tandis que le KD de Bim conduit à environ 60% de protection contre l’apoptose induite par cette combinaison de cytokines. La transcription de Bim est induite par STAT1 activé. Parallèlement à la régulation positive de Bim, TNF-α+IFN-γ conduit à la régulation négative de la protéine Bcl-XL. Bcl-XL est une protèine anti-apoptotique de la famille de protèines Bcl-2 qui en general inhibe Bim. Réduire l’expression de Bcl-XL seul induit une augmention de l'apoptose, alors que le KD de Bim et Bcl-XL en parallèle empêche l'apoptose.<p>Le but ultime de notre recherche est de protéger les cellules bêta des agressions autoimmunitaires. Les données antérieures ont révélé que JunB inhibe le stress du réticulum endoplasmique et l'apoptose dans les cellules bêta traitées avec IL-β+IFN-γ. Nous avons observé que TNF-α+IFN-γ induit l'expression de JunB qui se produit en aval de NF-ĸB activé. Il est important de noter que l’inactivation de JunB par des agents interférants de l’ARN (siRNA) exacerbe la mort des cellules primaires bêta de rat et de cellules INS-1E induite par les cytokines. Les réseaux de gènes touchés par JunB ont été étudiés grâce a l'analyse en microréseaux. JunB règule 20-25% des gènes modifiés par des cytokines dans les cellules bêta, y compris le facteur de transcription ATF3 et Bcl-XL. L’expression d’ATF3 est augmenté dans les îlots humains traités avec les cytokines et la répression in vitro de JunB conduit à une réduction de >60% de l’expression d’ATF3. Nous avons confirmé la régulation d’ATF3 par JunB en montrant que JunB est directement lié au promoteur d’ATF3 via le site ATF/CRE. La diminution d’expression d’ATF3 en presence de TNF-α+IFN-γ a aggravé la mort cellulaire induite dans les cellules bêta et a conduit à la régulation négative de l'expression de Bcl-XL dans les cellules INS-1E. L’augmentation pharmacologique de JunB dans les cellules INS-1E par l’utilisation de forskolin a conduit à la régulation positive en aval d’ATF3 et par conséquente à la protection de cellules bêta vis-a-vis de effets indésirables des cytokines. Dans cette optique, la surexpression génétique de JunB dans le modèle Ubi-JunB de souris transgénique a conduit à une surexpression d’ATF3 dans les îlots pancréatiques et a permir d’inverser les effets pro-apoptotiques de cytokines sur la cellule bêta (protection ± 40%).<p>Globalement, ces résultats indiquent que TNF-α+IFN-γ déclenche l'apoptose des cellules bêta par la régulation positive du gène pro-apoptotique Bim et la régulation négative du gène anti-apoptotique Bcl-XL. Ces effets indésirables sont inhibé en partie par JunB via l’activation de ATF3.<p><p>1Pas d’équivalent en français. Signifie la réduction de l’expression d’un gène via utilisation d’un siRNA (agent interférant de l’ARN).<p> / Doctorat en Sciences biomédicales et pharmaceutiques / info:eu-repo/semantics/nonPublished Disciplines biomédicales diverses Médecine pathologie humaine Transcription factors Islands of Langerhans Pancreatic beta cells Apoptosis Autoimmune diseases Facteurs de transcription Langerhans, Ilots de Langerhans, Cellules bêta des îlots de Apoptose Maladies auto-immunes STAT1 AP1 BCL-2 proteins transcription factors apoptosis beta cell
144	Suplementação alimentar com óleo de peixe reduz a expressão da NADPH oxidase e aumenta a expressão da SOD1 e SOD2 em ilhotas pancreáticas de ratos. / Fish oil supplemented diet reduces NAD(P)H oxidase expression and increases SOD-1 and SOD2 expression in rat pancreatic islets. Lucena, Camila Ferraz 21 September 2012 (has links) A secreção de insulina é estimulada pela glicose, porém os ácidos graxos (AG) podem influenciar o processo secretório. A oxidação de AG é importante para a estimulação da secreção de insulina por aumentar o ATP, porém, existem vias dependentes e independentes de ATP. Os AG <font face=\"Symbol\">w-3 interferem em processos fisiológicos e na composição e função da membrana plasmática, promovendo potente ação anti-inflamatória. Considerando a importante relação da NAD(P)H oxidase com a secreção de insulina, o estudo das alterações induzidas pela suplementação com AG <font face=\"Symbol\">w-3 sobre o conteúdo de superóxido (O2<font face=\"Symbol\">·) e a expressão da NAD(P)H oxidase, é importante para a compreensão da fisiologia das células <font face=\"Symbol\">b-pancreáticas. Neste estudo, o grupo suplementado apresentou redução do conteúdo de O2<font face=\"Symbol\">·, redução da expressão das subunidades da NAD(P)H oxidase e aumento na expressão da superóxido dismutase (SOD1 e 2), quando comparado ao grupo controle. Embora desconhecido o mecanismo, este dado é relevante, pois pressupõe melhor regulação do estado redox durante a secreção de insulina. / Insulin secretion is stimulated by glucose (GSIS), but fatty acid (FA) may influence the secretory process. The oxidation of FA is important for the stimulation of insulin secretion by increasing the ATP, although there are dependent and independent ATP pathways. The <font face=\"Symbol\">w-3 FA change physiological processes, and affect the composition and function of the plasma membrane, promote potent anti-inflammatory action. Considering the important relationship of NAD(P)H oxidase with insulin secretion, the study of changes induced by supplementation with <font face=\"Symbol\">w-3 FA on the superoxide (O2<font face=\"Symbol\">·) content, and expression of NAD(P)H oxidase, becomes of great importance for understanding the pancreatic <font face=\"Symbol\">b cells physiology. In this study, the group supplemented with <font face=\"Symbol\">w-3 FA showed a reduction of the O2<font face=\"Symbol\">· content, reduced expression of NAD(P)H oxidase subunits, and increased the expression of the enzyme superoxide dismutase (SOD 1 and 2), compared to control. Although unknown the mechanism, this data is relevant, because it represents better regulation of the redox state during GSIS . Ácido graxo ômega 3 Fatty acids omega 3 Ilhotas de langerhans Insulin Insulina Islets of langerhans Superoxides dismutase Superóxidos dismutase Suplementação alimentar Supplementary feeding
145	Estudo da imunidade inata na rosácea: células de Langerhans, células dentríncas pasmocitóides, receptores toll-like e expressão da forma induzida da enzima óxido nítrico sintase em biópsias de pele / Inate immunity in rosacea: Langerhans cells, plasmacytoid dentritic cells, toll-like receptors and inducible oxide nitric synthase (iNOS) expression in skin specimens Moura, Ana Karina Alves 22 February 2013 (has links) Introdução: Rosácea é uma doença inflamatória cutânea crônica relativamente comum, com incidência que varia de 2 a 10%. Caracteriza-se pelo surgimento de pápulas e pápulo-pustulas, eritema e telangiectasias precedidas por episódios de flushing. Apesar de não ser doença que comprometa o estado geral dos doentes, por ter acometimento preferencial da face, representa problema estético acentuado que interfere na socialização e qualidade de vida dos doentes. A etiologia da rosácea permanece incerta. A participação da imunidade inata tem sido implicada recentemente. Objetivo: Este estudo avaliou o envolvimento da imunidade inata na patogenia da rosácea através de pesquisa de células de Langerhans, células plasmocitóides (PDC), receptores \"toll-like\" (TLR) e expressão da forma induzida da enzima óxido nítrico sintase (iNOS) em biopsias de pele de pacientes com diagnóstico de rosácea. Métodos: Biopsias de 28 pacientes com diagnóstico clínico e histopatológico de Rosácea foram classificadas de acordo com características histopatológicas em Rosácea Granulomatosa (RG) (n = 10) e Rosácea Não Granulomatosa (RNG) (n = 18), e submetidas à técnica imunoistoquímica para demonstração de células de Langerhans (anticorpo anti-CD1a) (n = 26), PCD (anticorpo anti- CD123) (n = 24) e expressão dos receptores toll-like 2 e 4, bem como da forma induzida da óxido nítrico sintase (iNOS) (n = 28). Todos foram comparados com controles de pele normal (n = 15). Resultados: A população de células de Langerhans epidérmicas foi menor no grupo rosácea. Foram encontradas PDC dérmicas isoladas ou agrupadas no grupo rosácea, representando um novo dado no estudo da sua etiopatogenia. A expressão de TLR 2, TLR 4 e iNOS foi maior no grupo rosácea do que no grupo controle, estando distribuída com forte predominância na epiderme e anexos. Não houve diferença dos achados entre os grupos RG e RNG. Conclusão: Demonstrou-se, pela primeira vez, a presença de PDC nas lesões de rosácea. Juntamente com os outros marcadores estudados, os resultados apresentados confirmam a participação da imunidade inata na patogênese da rosácea através de mecanismos interdependentes e associados / Introduction: Rosacea is a common, chronic inflammatory condition with a reported prevalence between 2 and 10%. The disease has a variety of clinical manifestations that include flushing, persistent erythema, papules, pustules and telangiectasia. Because the facial skin is the predominant site of involvement, many patients sense that rosacea alters their social interactions affecting quality of life. The etiology of rosacea remains unknown. Recent studies have suggested that aberrant innate immunity is central to this disease. Objective: The aim of the present study was to examine the presence of Langerhans cells, plasmacytoid dentritic cells (PDC), and the expression of toll-like receptors (TLR) and inducible oxide nitric synthase (iNOS) in skin of patients with rosacea, in order to highlight the participation of innate immunity in the pathogenesis of this disease. Methods: 28 biopsy specimens were taken from patients with clinical and histopathological findings of rosacea. The samples were classified as Granulomatous rosacea (GR) (n= 10) or Non-Granulomatous rosacea (NGR) (n =18) according to histopathological features. Immunohistochemical demonstration of Langerhans cells (anti-CD1a antibody) (n = 24), PDC (anti-CD 123 antibody) (n = 26), TLR 2, TLR 4 and iNOS (n = 28) was performed in skin samples. The results were compared to normal skin control group (n = 15). Results: The number of Langerhans cells was lower in rosacea group than in control group. PDC were found in skin samples of rosacea as isolated cells and forming small clusters which represents a new contribution to the researches of its etiology. Expression of TLR2, TLR4 and iNOS was higher in rosacea samples than in normal skin controls, predominatly located in epidermal and adnexal structures. The comparison between GR and NGR groups did not show significant statistical difference. Conclusion: This research demonstrates, for the first time, the presence of PDC in lesions of rosacea, which together with the other results of this study, ratifies the existence of an altered innate immunity in pathogenesis of rosacea Células de Langerhans Células dendríticas plasmocitóides Dendritic cells Immunity innate Imunidade inata Langerhans cells Nitric oxide synthase Óxido nítrico sintase Receptores toll-like Rosacea Rosácea Toll-like receptors
146	Efeito in vitro do deidroepiandrosterona (DHEA) sobre a via IRS/PI3-K/Akt e secreção de insulina em ilhotas pancreáticas de ratos. / Effect in vitro of dehydroepiandrosterone (DHEA) on IRS/PI3-K/Akt pathway and insulin secretion on rats pancreatic islets. Camporez, João Paulo Gabriel 28 April 2008 (has links) A administração de deidroepiandrosterona (DHEA) tem resultado em efeitos anti-diabetogênicos em animais de experimentação e no homem. Assim, o objetivo desse trabalho é avaliar o efeito do DHEA in vitro na expressão protéica do IR, do IRS-1, IRS-2, PI3-K, Akt, ERK-1/2; na expressão gênica do PDX-1, do PGC-1, da insulina, do GLUT-2 e da glicocinase; e avaliar a secreção estática de insulina de ilhotas pancreáticas de ratos. O cultivo das ilhotas por 24 horas com DHEA, não induziu nenhuma alteração tanto na expressão das proteínas quanto na secreção estática de insulina estimulada por glicose. Ocorreu aumento da fosforilação de ERK-1/2 e na expressão gênica do PGC-1. As células RINm5F, cultivadas por 72 horas com DHEA, apresentaram aumento da expressão total de IRS-1 e IRS-2. Concluímos, que 24 horas de cultura com ilhotas não é tempo suficiente para observar nenhuma alteração induzida pelo DHEA, na secreção de insulina, e na expressão das proteínas da via IRS/PI3-K/Akt. Células RINm5F podem ser um modelo alternativo para investigar os efeitos diretos do DHEA. / The dehydroepiandrosterone (DHEA) administration has resulted in reduction of abdominal fat and protection against insulin resistance from experimental animals and humans. So, the purpose of this project is measure the in vitro effects from DHEA: on protein expression of insulin receptor, the proteins IRS-1, IRS-2, PI3-K, Akt, and ERK-1/2; on gene expression of transcriptional factors PDX-1 and PGC-1, insulin, glucose transport GLUT-2 and glicocinase; and to measure the static insulin secretion, on cultured pancreatic islets of the rat. The culture of pancreatic islet for 24 hours with DHEA, did not induce nothing alteration on protein expression of the IR, IRS-1, IRS-2, PI3-K, Akt-1 and ERK-1/2, and static insulin secretion induced by glucose. However, happened increase ERK-1/2 phosphorylation and PGC-1 gene expression. The RINm5F cells, cultured by 72 hours, showed increase of the IRS-1 and IRS-2 expression. We conclude that 24 hours of the pancreatic islets culture are not sufficient time to look any alteration induced by DHEA, on insulin secretion, and on protein expression involved on IRS/PI3-K/Akt pathway. RINm5F cells can be an alternative model to research the direct effects from DHEA. Diabetes Mellitus Diabetes Mellitus Expressão gênica Gene expression Homônios sexuais Ilhotas de Langerhans Insulin receptor Insulin signaling Langerhans islets Receptores da insulina Sexual hormone Sinalização da insulina
147	Modulação redox, função e sobrevivência de células β-pancreáticas: evidência sobre o papel da enzima NADPH oxidase-2 (NOX2) em um modelo in vitro de glicotoxicidade. / Redox modulation, function and survival of pancreatic β-cells: evidence on the role of NADPH oxidase-2 (NOX2) enzyme in a model of glucotoxicity in vitro. Souza, Arnaldo Henrique de 09 May 2016 (has links) O estresse oxidativo e a enzima NADPH oxidase-2 (NOX2) estão associados com a diminuição da massa funcional de células-β em pacientes com diabetes do tipo 2 (DT2). Neste estudo, testamos o papel da NOX2 sobre a glicotoxicidade em células-β. Ilhotas de camundongo C57BL/6J nocautes ou não para NOX2 (NOX2-KO e WT, respectivamente) foram isoladas e cultivadas por até 3 semanas em 10 ou 30 mmol/l de glucose (G10 e G30, respectivamente). A secreção de insulina foi maior nas ilhotas NOX2-KO vs. WT sem apresentar diferenças metabólicas ou do potencial redox da glutationa citosólica (EGSH). O cultivo de ilhotas em G30 aumenta a concentração de H2O2 e a oxidação de tióis no compartimento citosólico, seguido por aumento de apoptose de células-β, mas, preservando a reposta máxima secretória. Estas respostas foram quase idênticas em ambos os tipos de ilhotas. Em conclusão, a NOX2 regula negativamente a secreção de insulina em ilhotas de camundongos C57BL/6J, mas não é um componente crítico para a sobrevivência de células β em um modelo in vitro de glicotoxicidade. / Oxidative stress and NADPH oxidase-2 (NOX2) enzyme are associated to the decline of the functional β-cell mass in type 2 diabetes (T2D). Here, we tested the role of NOX2 on β-cell glucotoxicity. NOX2 knockout (NOX2 KO) and wild type (WT) C57BL/6J mice islets were isolated and cultured up to 3 weeks at 10 or 30 mmol/l glucose concentrations (G10 and G30, respectively). The insulin secretion was higher in NOX2-KO vs. WT islets despite similar metabolic and cytosolic glutathione-redox potential (EGSH) changes. The prolonged culture at G30 increases the H2O2 concentration and cytosolic thiol oxidation, followed by increased βcell apoptosis but preserving maximal secretory response. These responses were almost identical in both types of islets. In conclusion, NOX2 is a negative regulator of insulin secretion in C57BL/6J mouse islets, but is not a critical component for β-cell survival in a model of glucotoxicity in vitro. β-cell Apoptose Apoptosis Célula-β Ilhotas de Langerhans Insulin Insulin secretion Insulina Islets of Langerhans NADPH oxidase NADPH oxidase NOX2 NOX2 roGFP roGFP Secreção de insulina
148	Estudo comparativo da pele pré e pós-laser fracionado minimamente ablativo com Erbium-YAG de 2940nm para tratamento de rítides da região perioral: avaliação clínica, anátomo-patológica e imuno-histoquímica / Comparative study of skin pre and post fractional photothermolysis with Erbium-YAG 2940nm for the treatment of perioral wrinkles: a clinical, histological and immunohistochemical analysis Odo, Lilian Mayumi 24 March 2010 (has links) Atualmente existem diversas opções terapêuticas para o tratamento do fotoenvelhecimento cutâneo.Uma das formas de tratamento muito utilizada é a fototerapia com laser. Com o desenvolvimento da tecnologia em lasers surgiu um novo conceito de tratamento da pele envelhecida, a fototermólise fracionada microablativa. Essa tecnologia fracionada visa combinar os efeitos visíveis de uma terapia ablativa com o conforto e segurança dos métodos não ablativos. Antes de atingir a pele o laser passa por uma lente óptica especial que o divide em microrraios. Tal procedimento produz colunas de lesões térmicas microscópicas que penetram na epiderme e derme, sem danificar o tecido circunvizinho. A grande vantagem de ser fracionado é que a pele íntegra ao redor de cada coluna funciona como um reservatório de células potentes para a rápida cicatrização e regeneração da pele, culminando com a produção de colágeno e resultando em uma pele mais jovial, sem o inconveniente de um longo período de recuperação pós-tratamento. 20 pacientes foram selecionadas para o tratamento das rítides periorais com uma sessão de laser Erbium-YAG de 2940nm, fracionado. Após 28 dias do procedimento observou-se melhora na textura da pele, clareamento de manchas e atenuação de rugas finas periorais. Foi realizado um estudo comparativo da quantificação das células de Langerhans e receptores toll-like ( TLRs ) 2, 3 e 9 na epiderme, antes e após 3, 7, 14 e 28 dias do tratamento e da quantificação das fibras de colágeno na derme superior, antes e após 28 dias do laser. Houve diferenças estatisticamente significativas entre as medianas dos valores de CD1a (p = 0,0085), TLR 2 (p = 0,0108), TLR 3 (p = 0,0011) e TLR 9 (p = 0,0012) na epiderme pré e pós-tratamento. Foi constatado que a significância se deu entre os valores: antes e após 14 dias para CD1a (diminuição), antes e após 7 dias para TLR 2 (diminuição), antes e após 14 dias para TLR 3 (aumento), antes e após 7 dias para TLR 9 (diminuição). Não se encontraram diferenças estatisticamente significativas entre os valores medianos das fibras colágenas do tipo I (p = 1,0000) e III (p = 0,3125) antes e após 28 dias do tratamento. O protocolo desse estudo mostrou-se bastante seguro, pois apresentou efeitos colaterais transitórios e nenhuma complicação permanente. / There are several treatment options for skin photoaging. One of them widely used nowadays is lasertherapy. The development of lasers technology introduced a new therapeutic concept for aging skin: ablative fractional photothermolysis. This technology combines the visible effects of an ablative therapy with the comfort and safety of nonablative methods. Before reaching the skin the laser passes through a special optical lens that splits it into tiny rays. This procedure produces columns of microscopic thermal injuries that penetrate the epidermis and dermis, without damaging the surrounding tissue. The great advantage of the fractional photothermolysis is that the intact skin around each column acts as a potent reservoir of cells for fast healing and skin regeneration, resulting in collagen production and a youthful skin without the inconvenience of a long period of recovery after treatment. 20 patients were selected for perioral wrinkles treatment with a session of fractional Erbium-YAG 2940nm. After 28 days of the procedure the perioral skin showed improvement in texture, bleaching of sunspots and attenuation of superficial wrinkles. A comparative study was conducted between the expression of Langerhans cells and toll-like receptors 2, 3 and 9 in the epidermis, before and after 3,7,14 and 28 days of treatment and among collagen fibers in the dermis, before and after 28 days of the laser. There were statistically significant differences between the median values of CD1a (p = 0.0085), TLR 2 (p = 0.0108), TLR 3 (p = 0.0011) and TLR 9 (p = 0.0012) in the epidermis pre and post-treatment. The significance occurred between the values: before and after 14 days for CD1a (decrease) before and after 7 days to TLR 2 (decrease) before and after 14 days for TLR 3 (increase) before and after 7 days for TLR 9 (decrease). There were not statistically significant differences between the median values of collagen type I (p = 1.0000) and III (p = 0.3125) before and after 28 days of treatment. The irradiation of skin with fractional Erbium-YAG was safe, as it showed transitory side effects and no permanent complication. Células de Langerhans Envelhecimento da pele Fototerapia Immunohistochemistry Imunoistoquímica Langerhans cells Laser Laser Pele Phototherapy Receptores Toll-like Skin Skin aging Toll-Like receptors
149	Interação do Paracoccidioides brasiliensis com células dendríticas e queratinócitos em biopsias de lesões de pele e mucosa oral / Paracoccidioides brasiliensis interacts with dermal dendritic cells and keratinocytes in human skin and oral mucosa lesions Silva, Wellington Luiz Ferreira da 25 May 2016 (has links) A paracoccidioidomicose (PCM) é uma doença sistêmica causada pelos fungos Paracoccidioides brasiliensis e Paracoccidioideslutzii. O comprometimento da pele e mucosa oral são frequentes na PCM. As células dendríticas e queratinócitos do tegumento, devido à sua função como células apresentadoras de antígenos, atuam na resposta imune inata e adaptativa contra agentes patogênicos. Com o objetivo de verificar a interação do P. brasiliensis com essas células, estudamos 47 biopsias de mucosa oral e 52 de pele de lesões de doentes com diagnóstico comprovado de PCM. As biopsias foram submetidas à técnica de imuno-histoquímica de dupla-marcação com os anticorpos anti-fator XIIIa (marcador de dendrócitos dérmicos), anti-CD207 (marcador de células de Langerhans maduras), anti-pancitoqueratinas (AE1-AE3) e anti-P. brasiliensis. Fez-se também a reação de dupla marcação por técnica de imunofluorescência, com análise por microscopia confocal a laser, para a melhor visualização da interação entre queratinócitos e os fungos. Quarenta e dois por cento das amostras de mucosa oral exibiram formas fúngicas no citoplasma de dendrócitos dérmicos. As células de Langerhans, tanto nas biopsias de mucosa oral como de pele, não mostraram leveduras ou antígenos do fungo no seu citoplasma. Cinquenta e quatro por cento das biopsias de pele e sessenta por cento das amostras de mucosa exibiram leveduras no citoplasma de queratinócitos. Os resultados obtidos permitem concluir que o parasitismo de queratinócitos pode representar possível mecanismo de evasão do fungo aos mecanismos imunes locais. Os dendrócitos dérmicos fator XIIIa positivos e queratinócitos podem estar a atuar como células apresentadoras de antígenos para suprir a função, provavelmente prejudicada, das células de Langerhans nas lesões de pele e mucosa oral da PCM humana / Paracoccidioidomycosis (PCM) is a systemic disease caused by the fungus Paracoccidioides brasiliensis, which compromises various organs, mainly the lungs. The skin and oral mucosa are often affected. Dendritic cells and keratinocytes of the integument play a role in innate and adaptive immune response against pathogens, due to their function as antigen presenting cells. Aiming to verify the interaction of P. brasiliensis with these cell populations, we studied 52 biopsies of skin and 47 oral mucosa samples taken from patients with proven diagnosis of PCM. The biopsies were subjected to double immune staining technique with anti-factor XIIIa (marker of dermal dendrocytes), anti- CD207 (marker of mature Langerhans cells), anti-pan cytokeratins (AE1-AE3) and anti P. brasiliensis antibodies. Analyses with confocal laser microscopy were also performed to better visualization of the interaction between keratinocytes and the fungi. Factor XIIIa + dermal dendrocytes of 42% samples of oral mucosa displayed yeast forms in their cytoplasm. We did not observe yeast cells in the cytoplasm of Langerhans cells in both skin and oral mucosa samples. Fifty -four percent of skin and 60% of mucosal samples displayed yeast cells in the cytoplasm of keratinocytes. The parasitism of keratinocytes may represent a possible mechanism of evasion of the fungus to local immune mechanisms, or even as a result of keratinocytes ability to antigen presentation in PCM. Factor XIIIa dendrocytes and keratinocytes may be acting as antigenpresenting cells to fulfill the function of Langerhans cells, probably impaired, in skin and mucosa of human PCM Células de Langerhans Células dendríticas Confocal microscopy Dendritic cells Immunohistochemistry Imuno-histoquímica Keratinocytes Microscopia confocal Mouth mucosa Mucosa bucal Paracoccidioidomicose Paracoccidioidomycosis Pele Queratinócitos Skin, Langerhans cells
150	Protective mechanism(s) of anti-oxidants in pancreatic-islet β-cells against glucose toxicity and oxidative stress. / Protective mechanism(s) of anti-oxidants in pancreatic-islet beta-cells against glucose toxicity and oxidative stress January 2011 (has links) Poon, Chui Wa Christina. / "August 2011." / Thesis (M.Phil.)--Chinese University of Hong Kong, 2011. / Includes bibliographical references (leaves 123-131). / Abstracts in English and Chinese. / ABSTRACT --- p.i / 論文摘要 --- p.vi / ACKNOWLEDGEMENTS --- p.ix / PUBLICATIONS --- p.x / Abstracts --- p.x / ABBREVIATIONS --- p.xii / Chapter 1. --- GENERAL INTRODUCTION --- p.1 / Chapter 1.1. --- Diabetes --- p.1 / Chapter 1.1.1. --- Overview --- p.1 / Chapter 1.1.2. --- Diagnostic Criteria of Type-2 Diabetes --- p.2 / Chapter 1.1.3. --- Type-2 Diabetes (T2DM) --- p.3 / Chapter 1.1.3.1. --- Impaired Insulin Synthesis and Insulin Secretory Defects in Type-2 Diabetes --- p.3 / Chapter 1.1.3.2. --- β-Cell Dysfunction --- p.5 / Chapter 1.1.3.3. --- Insulin Resistance --- p.5 / Chapter 1.1.4. --- Glucose Toxicity --- p.6 / Chapter 1.1.4.1. --- Fasting Hyperglycemia --- p.8 / Chapter 1.1.4.2. --- Postprandial Hyperglycemia --- p.8 / Chapter 1.2. --- Oxidative Stress --- p.8 / Chapter 1.2.1. --- ROS and Mitochondria --- p.8 / Chapter 1.2.2. --- ROS Production by Mitochondria --- p.9 / Chapter 1.2.3. --- The Relationship of Glucose Recognition by β-cells and Oxidative Stress --- p.11 / Chapter 1.2.4. --- Important Roles of Glutathione in Pancreatic β-cells and Glutathione Synthesis --- p.14 / Chapter 1.2.5. --- N-acetyl-L-cysteine - A Potential Drug Treatment for Type-2 Diabetes? --- p.17 / Chapter 1.3. --- Role of F-actin Cytoskeleton on Glucose-induced Insulin Secretion --- p.18 / Chapter 1.4. --- Current Clinical Treatments for Type-2 Diabetes Mellitus --- p.21 / Chapter 1.4.1. --- Metformin --- p.22 / Chapter 1.4.2. --- Sulfonylureas --- p.22 / Chapter 1.4.3. --- Thiazolidinediones --- p.23 / Chapter 1.4.4. --- Glinides (Meglitinide Analogues) --- p.23 / Chapter 1.4.5. --- α-Glucosidase (AG) Inhibitors --- p.24 / Chapter 1.4.6. --- Dipeptidyl Peptidase-4 (DPP-4) Inhibitors --- p.24 / Chapter 1.4.7. --- (Clinical) Antioxidant Treatment --- p.24 / Chapter 1.5. --- Animal Models Used in Type-2 Diabetes Research --- p.25 / Chapter 1.6. --- Aims of Study --- p.27 / Chapter 2. --- RESEARCH DESIGN & METHODS --- p.28 / Chapter 2.1. --- Materials --- p.28 / Table 1. Sources and concentrations of drugs tested in this study: --- p.28 / Culture Medium - --- p.29 / General Reagents --- p.29 / Chapter 2.2. --- Isolation of Islets of Langerhans and Single Pancreatic β-Cells --- p.31 / Chapter 2.3. --- Measurement of Mitochondrial ROS Levels --- p.32 / Chapter 2.4. --- Measurement of Islets Insulin Release and Insulin Content --- p.34 / Chapter 2.4.1. --- Preparation of Samples --- p.34 / Chapter 2.4.2. --- Enzyme-Link Immunosorbent Assay (ELISA) --- p.35 / Chapter 2.5. --- Immunocytochemistry --- p.35 / Chapter 2.6. --- Data and Statistical Analysis --- p.37 / Chapter 3. --- RESULTS --- p.38 / Chapter 3.1. --- "Effects of L-NAC, Various Oxidative Stress Inducers/Reducers and Actin Polymerisation/Depolymerisation Inducers on Releasable Insulin Levels and Insulin Contents in Response to Low Glucose (5 mM) and High Glucose (15 mM) of Isolated Pancreatic Islets of (db+/m+) and (db+/db+) Mice" --- p.38 / Chapter 3.1.1. --- Effect of L-NAC on Insulin Secretion and Insulin Contents --- p.38 / Chapter 3.1.2. --- Effect of Cytochalasin B on Insulin Secretion and Insulin Contents --- p.39 / Chapter 3.1.3. --- Effect of 4-Phenyl Butyric Acid on Insulin Secretion and Insulin Contents --- p.43 / Chapter 3.1.4. --- Effect of Ursodeoxycholic Acid on Insulin Secretion and Insulin Contents --- p.46 / Chapter 3.1.5. --- Effect of Hydrogen Peroxide on Insulin Secretion and Insulin Contents --- p.49 / Chapter 3.1.6. --- Effect of Jasplakinolide on Insulin Secretion and Insulin Contents --- p.53 / Chapter 3.1.7. --- Effect of Thapsigargin on Insulin Secretion and Insulin Contents --- p.57 / Chapter 3.1.8. --- Effect of BSO on Insulin Secretion and Insulin Contents --- p.61 / Chapter 3.2. --- "Effects of L-NAC, Various Oxidative Stress Inducers/Reducers and Actin Polymerisation/Depolymerisation Inducers on Mitochondrial ROS Levels in Response to High Glucose (15 mM) Challenge in Isolated Single Pancreatic β-Cells of (db +/m+) and (db +/db +) Mice" --- p.65 / Chapter 3.2.1. --- "Effects of L-NAC (20 mM), 4-Phenyl Butyric Acid (4-PBA) (1 mM), Ursodeoxycholic Acid (UA) (500 μg/ml), H202 (200 μM), Thapsigargin (0.5 μM) and DL-Buthionine-[S,R]-Sulfoximine (BSO) (0.1 μM) Pre-treatments on Mitochondrial ROS Level in Response to High Glucose (15 mM) Challenge" --- p.65 / Chapter 3.2.2. --- "Effects of L-NAC (20 mM), Cytochalasin B (10 μM) and Jasplakinolide (5 μM) Pre-treatments on Mitochondrial ROS Level in Response to High Glucose (15 mM) Challenge_" --- p.76 / Chapter 3.3. --- "Effects of L-NAC, Various Oxidative Stress Inducers/Reducers and Actin Polymerisation/Depolymerisation Inducers on F-actin Cytoskeleton Levels Incubated in Low Glucose (5 mM) and High Glucose (15 mM) Medium in Single Pancreatic β-Cells of Non-Diabetic (db +/m+) and Diabetic (db +/db +) Mice" --- p.81 / Chapter 4. --- DISCUSSION --- p.100 / Chapter 4.1. --- General Discussion --- p.100 / Chapter 5. --- SUMMARY --- p.120 / Chapter 6. --- FUTURE PERSPECTIVES --- p.121 / Chapter 7. --- REFERENCES --- p.123 Antioxidants--Therapeutic use Islands of Langerhans--Physiology Pancreatic beta cells Oxidative stress Antioxidants--therapeutic use Islets of Langerhans--physiology Oxidative Stress Diabetes Mellitus, Type 2--complications

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