Impact du statut de différenciation des cellules promyélocytaires HL-60 sur l’efficacité anticancéreuse et antiinflammatoire de l’EGCG

Vézina, Amélie

05 1900

L’altération de la barrière hématoencéphalique (BHE) par les cellules tumorales et les cellules immunes circulantes peut mener à la neuroinflammation. Les cellules leucémiques promyélocytaires HL-60 sont un excellent modèle pour étudier et comprendre les mécanismes de signalisation moléculaires qui caractérisent le développement tumoral et métastatique. La cancérogenèse peut s’accompagner de modulations de l’expression de biomarqueurs tels que la cyclooxygénase-2 et la métalloprotéase-9. Les recherches décrites dans ce mémoire relatent l’analyse des biomarqueurs inflammatoires et invasifs régulés lors de la différenciation induite par le PMA des cellules HL-60 en macrophages. Le statut de différenciation cellulaire pourrait avoir un impact sur les gènes cibles de la voie NF-κB. Nous émettons l’hypothèse que le PMA active la voie NF-κB et que cette signalisation peut être renversée par l’(-)-épigallocatéchine-gallate (EGCG). En effet, une régulation à la hausse de l’expression de plusieurs gènes combinée à la diminution de l’expression d’IκB mettent en évidence l’implication de la voie NF-κB dans l’activation des mécanismes pro-inflammatoires et pro-invasifs. Les mêmes observations sont faites dans les cellules différenciées appelées «macrophages-like». L’EGCG, un polyphénol dérivé du thé vert, a un potentiel chimiopréventif. Il est capable d’inhiber la signalisation moléculaire passant par la voie NF-κB dans les cellules HL-60 traitées simultanément par l’EGCG et le PMA, mais pas dans les cellules «macrophages-like». Cette différence peut s’expliquer par une modulation de l’expression du récepteur de surface cellulaire de l’EGCG, le récepteur à la laminine de 67 kDa, et de son précurseur de 37 kDa. Collectivement, nos résultats montrent que le statut de différenciation des cellules promyélocytaires HL-60 concorde avec l’activation des mécanismes favorisant le développement d’un cancer et des métastases. Cet effet peut être prévenu par l’utilisation d’agents naturels tel l’EGCG. Le ciblage de biomarqueurs liés au statut de différenciation des cellules tumorales impliquées dans la perturbation de la barrière hématoencéphalique qui cause la neuroinflammation permettrait l’avancement des connaissances dans la prévention de la cancérogenèse. / Blood-brain barrier (BBB) disruption by circulating tumor and immune cells leads to secondary inflammatory infections. Promyelocytic HL-60 cells represent an excellent model to study and to get a better understanding of the molecular signaling mechanisms involved in carcinogenesis and metastasis. The research described in this thesis shows the analysis of several inflammatory and invasive biomarkers regulated during PMA-induced differentiation of promyelocytic HL-60 cells into macrophages. Carcinogenesis involves some modifications in the expression of biomarkers such as cyclooxygenase-2 and matrix metalloprotease-9. The differentiation status could have an impact on the NF-κB signaling pathway that regulates the target genes, given that these target genes expression varies during cell differentiation. We hypothesize that the activation of the NF-κB pathway by PMA can be reverse by (-)-epigallocatechin-gallate (EGCG). Indeed, the up-regulation of downstream genes combined with the down-regulation of IκB expression showed the significant implication of the NF-κB signaling pathway to activate pro-inflammatory and pro-invasive mechanisms linked to carcinogenesis. The same evidence exhibits in the differentiated cells called «macrophages-like». Moreover, the green tea polyphenol, EGCG, shows chemopreventive property since it better inhibited NF-κB signaling in cells treated simultaneously with EGCG and PMA compared to the «macrophages-like». This difference could be due, in part, to the down-regulation of the 67 kDa laminin receptor, known to be the non-integrin membrane receptor for EGCG. All together, our results suggest that the differentiation status of promyelocytic cells is linked to the activation of mechanisms involved in carcinogenesis and metastasis. These phenomena can be prevented by using natural agents such as EGCG. Targeting the specific biomarkers linked to the differentiation status of tumor cells and involved in the disruption of the BBB may help reduce secondary neuroinflammation and enable the advancement of knowledge towards carcinogenesis prevention.

cellules HL-60

inflammation

cyclooxygénase-2

métalloprotéase matricielle (MMP-9)

NF-kB

(-)-épigallocatéchine-3-gallate

HL-60 cells

cyclooxygenase-2

matrix metalloprotease

(-)-epigallocatechin-3-gallate

Impact des cavines sur le phénotype invasif et inflammatoire des cellules souches mésenchymateuses

Annabi, Bayader

03 1900

L’évolution d’une cellule tumorale initiée à une tumeur solide nécessite, à chaque étape, un microenvironnement favorable à sa survie et à sa croissance. Le microenvironnement tumoral est comparé à un foyer d’inflammation chronique dont la composition cellulaire et moléculaire est complexe. Les cellules souches mésenchymateuses (CSM) représentent l’un des principaux acteurs cellulaires présents. Elles migrent vers les sites tumoraux où elles soutiennent l’inflammation, l’angiogenèse et le développement tumoral en activant plusieurs voies de signalisation. Une des voies majeures qui contribuent à l’inflammation est la voie de signalisation NF-B. L’initiation de cette voie provient de la membrane cellulaire entre autres des cavéoles. Nous soumettons l’hypothèse que l’une des cavines, protéines associées aux cavéoles, modulerait le phénotype inflammatoire etou migratoire dans les CSM traitées à la cytokine TNF- (facteur de nécrose tumorale ) en modulant la voie de signalisation NF-B. En effet, nous avons observé une régulation à la hausse de l’expression de la COX-2 (cyclooxygénase-2) et une diminution de l’expression d’IκB qui sont synonymes de l’activation de la voie NF-B dans les CSM que nous avons traitées au TNF-. Nous avons trouvé que le TNF- induit la migration des CSM, et que la répression génique de la Cavine-2 augmente significativement la migration des CSM traitées par le TNF-. La répression génique de la Cavine-2 vient aussi amplifier la tubulogenèse dans les CSM en réponse au TNF-. D’un point de vue moléculaire, la répression génique de la Cavine-2 a montré une très forte amplification de l'expression protéique de la COX-2 dans les CSM en réponse au TNF-. Dans ces mêmes cellules où la Cavine-2 a été réprimée, et suite à un traitement au TNF-, le pic de phosphorylation est plus intense et la courbe de phosphorylation est plus prolongée dans le temps. Ces observations nous permettent d’affirmer que la Cavine-2 a un rôle répresseur sur l’expression de COX-2. Collectivement, nos résultats montrent que la Cavine-2 peut être proposée comme un gène suppresseur de tumeur et est de ce fait, une bonne cible thérapeutique dans les CSM qui permettraient d’agir à des stades précoces du développement tumoral. / The evolution of an initiated tumor cell into a solid tumor requires at each stage a favorable microenvironment for its survival and growth. The tumor microenvironment is compared to a chronic inflammation site with a cellular and molecular complex composition. Mesenchymal stem cells (MSC) have important roles in tumor microenvironment. They migrate to tumor sites where they maintain the inflammation, angiogenesis and tumor development by activating multiple signaling pathways. One of the major pathways that contribute to inflammation is the NF-B signaling pathway. The initiation of this pathway comes from the cell membrane and caveolae. Our hypothesis is that one of cavins, proteins associated to caveolae, modulates the inflammatory phenotype and migration in MSC treated with TNF-. We suggest that this process is modulated by a NF-B signaling pathway. Indeed, we observed an up-regulation of the expression of the cyclooxygenase-2 (COX-2) and a decrease in the expression of IκB which suggest that activation of the NF-B pathway is involved in the MSC treated with TNF. We found that the TNF- induced migration in the MSC, and the knockout of Cavin-2 significantly increased migration of MSC treated with TNF-. The silencing of Cavin-2 considerably increased tubulogenesis of MSC treated with TNF-. At the molecular level, knockout of Cavin-2 showed a very strong amplification of protein expression of COX-2 in the MSC in response to TNF-. In these same cells where Cavin-2 was repressed and treated with TNF-, the peak of phosphorylation of pIB is more intense and the phosphorylation curve is sustained in time. These observations allow us to assert that Cavin-2 has a repressing role on the expression of COX-2. Collectively, our results show that the gene encoding Cavin-2 can be proposed as tumor suppressor gene. This study allowed us to identify new therapeutic targets: Cavins proteins.

Cellules souches mésenchymateuses

Cavines

Inflammation

Migration

TNF-alpha

COX-2

NF-κB

mesenchymal stem cells

cavins

inflammation

migration

TNF-aplha

COX-2

NF-kB

A Novel Role for the TRAFs as Co-Activators and Co-Repressors of Transcriptional Activity

Brittain, George C. IV

16 June 2009

The tumor necrosis factor (TNF) receptor-associated factors (TRAFs) were initially discovered as proteins that inducibly interact with the intracellular region of TNF receptors (TNFRs). Because the TNFRs lack intrinsic catalytic activity, the TRAFs are hypothesized to orchestrate signaling activation downstream of the TNFR superfamily, however their mechanism of activation remains unclear (Inoue et al., 2000; Bishop, 2004). Originally, the TRAFs were compared to the signal transducers and activators of transcription (STAT) protein family, due to their sequence homology, and the presence of multiple RING- and zinc-finger domains, suggesting that their function may be to regulate transcriptional activity (Rothe et al., 1994; Hu et al., 1994; Sato et al. 1995; Cheng et al., 1995). However, subsequent research focused predominantly on their cytoplasmic functions, and more recently on their function as E3 ubiquitin ligases (Pineda et al., 2007). In my research, I analyzed the subcellular localizations of the TRAFs following CD40 ligand (CD40L)-stimulation, and found that TRAF2 and 3 rapidly translocate into the nucleus of primary neurons and Neuro2a cells. Interestingly, similar analysis conducted in pre-B lymphocytes (Daudi cells) revealed a different response to CD40L-stimulation, with TRAF2 and 3 being rapidly degraded within 5-minutes of stimulation. These findings are significant because they demonstrate for the first time that the TRAFs translocate into the nucleus and suggest that they may function within the nucleus in a cell-specific manner. I next analyzed the ability of TRAF2 and 3 to bind to DNA, and found that they both bind to chromatin and the NF-kappaB consensus element in Neuro2a cells, following CD40L-stimulation. Similar analyses of the chromatin binding of TRAF2 and 3 in Daudi cells revealed that they were rapidly degraded, similar to the results from my analysis of their subcellular localization. These findings show for the first time that the TRAFs interact with DNA, and therefore support the hypothesis that the TRAFs may function within the nucleus as transcriptional regulators. Finally, I analyzed the ability of the TRAFs to regulate transcriptional activity by luciferase assay. Previous studies showed that overexpression of TRAF2 and 6 could induce NF-kappaB transcriptional activity; however researchers have not been able to determine the mechanism by which they do so. In my studies, I found that every TRAF can directly regulate transcriptional activity either as co-activators or co-repressors of transcription, in a cell- and target protein-specific manner. Additionally, I found that TRAF2 can act as a transcriptional activator, and that its ability to regulate transcription is largely dependent upon the presence of its RING-finger domain. In conclusion, these studies have revealed an entirely novel function for the TRAFs as immediate-early transcriptional regulators. Future research into the genes that are regulated by the specific TRAF complexes will further elucidate how the TRAFs regulate TNFR signaling, as well as whether dysfunctions in TRAF signaling may be associated with known disorders. If specific TRAF complexes are found to regulate specific genes, then pharmacological targeting of the individual TRAF complexes may allow for the highly specific inhibition of signaling events downstream of the TNFRs, without compromising overall receptor signaling, transcription factor pathways, or cellular systems.

Japanese Encephalitis Virus Infection In Vitro : Role Of Type-I Interferons And NF-kB In The Induction Of Classical And Nonclassical MHC-I Molecules

Abraham, Sojan

01 1900

Japanese encephalitis virus (JEV) is one of the major causes of encephalitis in Asia. JEV causes serious inflammation of the brain, which may lead to permanent brain damage and has a high mortality rate. Almost 3 billion people live in JE endemic areas and JEV causes an estimated 20,000 cases of disease and 6000 deaths per year. JEV is a positive stranded RNA virus belonging to the Flavivirus genus of the family Flaviviridae. The genome of JEV is about 11 kb long and codes for a polyprotein which is cleaved by both host and viral encoded proteases to form 3 structural and 7 non-structural proteins. JEV transmission occurs through a zoonotic cycle involving mosquitoes and vertebrate amplifying hosts, chiefly pigs and ardeid birds. Humans are infected when bitten by an infected mosquito and are dead end hosts. The role of humoral and cell mediated immune responses during JEV infection have been studied by several groups. While the humoral responses play a central role in protection against JEV, the cell mediated immune responses contributing to this end are not fully understood. The MHC molecules have been known to play predominant roles in host responses to viral infections and the consequences of virus infection on the expression of MHC molecules are varied. The expression of MHC-I molecules is known to decrease upon infection with many viruses such as HIV, MCMV, HCMV, Adv, and EBV. In contrast, infection with flavivirus such as West Nile Virus (WNV) has been shown to increase the cell surface expression of both MHC-I and MHC-II molecules. It has been reported previously that WNV infection increases the cell surface expression of adhesion molecules such as ICAM-1, VCAM-1 as well as E-Selectin and these changes were mediated directly by WNV and not by soluble cytokines. In contrast to classical MHC-I molecules, the nonclassical MHC-I molecules do not belong to a single group of structurally and functionally homologous proteins and normally have lower cell surface expression. Earlier studies have shown that the expression of nonclassical MHC-I molecules were induced during infection with JHM strain of mouse hepatitis virus (MHV). However, the functional significance of this induction is unclear. Expression of nonclassical MHC-I molecules upon flaviviral infection is not very well understood. In this thesis, evidence is presented that JEV infection induces the expression of both classical and nonclassical MHC-I molecules on primary mouse brain astrocytes, mouse embryonic fibroblasts (MEFs) and H6 (hepatoma cell). The levels of adhesion molecules as well as molecules involved in antigen processing and presentation were also analyzed and our results clearly demonstrate that JEV infection induces their expression on astrocytes, MEFs and H6. The role of NF-κB and type-I IFNs in the induction of classical and nonclassical MHC-I molecules as well as molecules involved in antigen processing and presentation were also analyzed and our results demonstrated that type-I IFN mediated signaling is responsible for the induction of these molecules during JEV infection. Chapter 1 discusses the innate and adaptive immune system, the role of classical and nonclassical MHC molecules in the initiation of immune response and diverse strategies adapted by different viruses to evade the immune response. It also includes a detailed discussion about the IFN and NF-κB signaling pathways and their modulation by viral infection. Finally, the genome organization, epidemiology, transmission cycle, pathogenesis and pathology, clinical features, humoral as well as cell mediated immune response to JEV infection and the current vaccine status to JEV infection are briefly discussed. Chapter 2 describes the general materials and methods used in this study. It includes the details of the reagents and cell lines used in the experiments. It also discusses the various techniques such as RT-PCR, FACS analysis, EMSA and ELISA. Chapter 3 focusses on the validation of different knockout MEFs used in the study as well as confirming the purity of primary astrocyte cultures established from pub brains. The susceptibility of various cells to JEV infection has also been investigated. Our results confirmed the authenticity of all the cells and the purity of primary astrocyte cultures used in the study. Our results also indicated that all the cells used in the study are susceptible to JEV infection. Chapter 4 discusses the expression of MHC and related genes involved in immune response upon JEV infection of primary mouse brain astrocytes, MEFs and H6. Chapter 4 demonstrates for the first time that JEV infection induces the expression of nonclassical MHC-I or class Ib molecules namely Qa-1, Qb1 and T10 in addition to the induction of classical MHC-I molecules. In contrast to WNV, there was no increase in the cell surface expression of MHC-II molecules upon JEV infection of primary mouse brain astrocytes. JEV infection also induces the expression of adhesion molecules as well as molecules involved in antigen processing and presentation namely Tap1, Tap2, Tapasin, Lmp2, Lmp7 and Lmp10. Chapter 5 demonstrates that JEV infection induces NF-κB activation in astrocytes and MEFs. Studies using MEFs deficient in classical and alternate pathways of NF-κB activation indicate that JEV activates the classical pathway of NF-κB activation and is dependent on canonical lKKβ/IKK2 activity. JEV infection of astrocytes, MEFs and H6 induces the production of type-I IFNs. To determine the mechanism of type-I IFN induction during JEV infection, MEFs deficient in NF-κB signaling and IFN signaling were used. Results indicate that type-I IFN production in MEFs occurs by both NF-κB dependent and independent mechanisms. In contrast, the production of IFN-α was completely abrogated in IFNAR-\- MEFs whereas IFN-β production was greatly reduced. Production of type-I IFNs in IFNGR-\- MEFs is also reduced upon JEV infection but the reason for this is unclear. Chapter 6 demonstrates that JEV induced expression of classical MHC-I molecules occurs by type-I IFN mediated signaling. This result is in contrast to WNV infection, in which both NF-κB and type-I IFNs are involved in the induction of classical MHC-I molecules. Type-I IFNs were also shown to be involved in the induction of nonclassical MHC molecules namely, Qa-1 and Qb1 during JEV infection. In contrast, the expression of T10, another nonclassical MHC molecule occurs independent of type-I IFN signaling. The expression of molecules involved in antigen processing and presentation namely, Tap1, Tap2, Lmp2 and Lmp7 was type-I IFN-mediated, whereas the expression of Tapasin and Lmp10 was mediated by both type-I IFN dependent and independent mechanisms. The expression of VCAM-1 was dependent on NF-κB mediated signaling. Chapter 7 precisely describes the underlying mechanism of induction of MHC and various other related molecules and their significance during JEV infection. In addition, it also includes a working model for the induction of these molecules during JEV infection. In summary, this is the first study in which the mechanism of JEV mediated induction of classical as well as nonclassical MHC molecules has been studied in detail. This study clearly demonstrated that type-I IFNs are involved in the induction of classical and nonclassical MHC-I molecules during JEV infection. The functional significance of this JEV mediated induction of classical MHC-I molecules is unclear, but it has been proposed that this is to escape from the action of NK cells. The absence of MHC-II induction during JEV infection could be important because it may lead to the initiation of an immune response which is different from that induced during other viral infections which induce the expression of MHC-II molecules. In contrast to classical MHC-I molecules, the functional and biological significance of nonclassical MHC-I molecules are poorly studied. Nonclassical MHC-I molecules play an important role in bridging adaptive and innate immune response. So the nonclassical MHC molecules induced during JEV infection may play an important role in the initiation of immune response during JEV infection. The role these nonclassical MHC-I molecules in antigen presentation during JEV infection is not known. These nonclassical antigens are also recognized by NK and γδT cells, thus the expression of nonclassical MHC-I molecules during JEV infection might also confer a protective role.

Japanese Encephalitis Virus (JEV)

RNA Viruses

Major Histocompatibility Complex

Virus Infection

Cell Adhesion Molecules

Flaviviruses

Interferons

Viruses

Virus Diseases - Immunological Aspects

Japanese Encephalitis Virus Infection

Virus Induced Molecules

Nuclear Factor kB

JEV Infection

MHC-I

Virology

Role of intestinal epithelium in inflammatory bowel disease: effect of cytokines and glucocorticoids on CXCL8 and CXCL10 gene expression and NF-kB signalling in intestinal epithelial cell lines / Untersuchungen zur Rolle des Darmepithels bei chronisch entzündlichen Darmerkrankungen: Über den Einfluss von Zytokinen und Glucocorticoiden auf die Expression der Chemokine CXCL8 und CXCL10 und den NF-kB Signalweg in intestinalen Epithel-Zelllinien

Yeruva, Sunil

04 May 2007

No description available.

500 Naturwissenschaften

WF 000 Molekularbiologie

Gentechnologie

Mathematics and Natural Science

Glucocorticoiden

Chemokine

CXCL8

CXCL10

NF- B

Intestinalen epithelzell linen

Glucocorticoids

Chemokine

CXCL8

CXCL10

NF-kB

Intestinal epithelial cell lines

42.13 Molekularbiologie

Impact du statut de différenciation des cellules promyélocytaires HL-60 sur l’efficacité anticancéreuse et antiinflammatoire de l’EGCG

Vézina, Amélie

05 1900

L’altération de la barrière hématoencéphalique (BHE) par les cellules tumorales et les cellules immunes circulantes peut mener à la neuroinflammation. Les cellules leucémiques promyélocytaires HL-60 sont un excellent modèle pour étudier et comprendre les mécanismes de signalisation moléculaires qui caractérisent le développement tumoral et métastatique. La cancérogenèse peut s’accompagner de modulations de l’expression de biomarqueurs tels que la cyclooxygénase-2 et la métalloprotéase-9. Les recherches décrites dans ce mémoire relatent l’analyse des biomarqueurs inflammatoires et invasifs régulés lors de la différenciation induite par le PMA des cellules HL-60 en macrophages. Le statut de différenciation cellulaire pourrait avoir un impact sur les gènes cibles de la voie NF-κB. Nous émettons l’hypothèse que le PMA active la voie NF-κB et que cette signalisation peut être renversée par l’(-)-épigallocatéchine-gallate (EGCG). En effet, une régulation à la hausse de l’expression de plusieurs gènes combinée à la diminution de l’expression d’IκB mettent en évidence l’implication de la voie NF-κB dans l’activation des mécanismes pro-inflammatoires et pro-invasifs. Les mêmes observations sont faites dans les cellules différenciées appelées «macrophages-like». L’EGCG, un polyphénol dérivé du thé vert, a un potentiel chimiopréventif. Il est capable d’inhiber la signalisation moléculaire passant par la voie NF-κB dans les cellules HL-60 traitées simultanément par l’EGCG et le PMA, mais pas dans les cellules «macrophages-like». Cette différence peut s’expliquer par une modulation de l’expression du récepteur de surface cellulaire de l’EGCG, le récepteur à la laminine de 67 kDa, et de son précurseur de 37 kDa. Collectivement, nos résultats montrent que le statut de différenciation des cellules promyélocytaires HL-60 concorde avec l’activation des mécanismes favorisant le développement d’un cancer et des métastases. Cet effet peut être prévenu par l’utilisation d’agents naturels tel l’EGCG. Le ciblage de biomarqueurs liés au statut de différenciation des cellules tumorales impliquées dans la perturbation de la barrière hématoencéphalique qui cause la neuroinflammation permettrait l’avancement des connaissances dans la prévention de la cancérogenèse. / Blood-brain barrier (BBB) disruption by circulating tumor and immune cells leads to secondary inflammatory infections. Promyelocytic HL-60 cells represent an excellent model to study and to get a better understanding of the molecular signaling mechanisms involved in carcinogenesis and metastasis. The research described in this thesis shows the analysis of several inflammatory and invasive biomarkers regulated during PMA-induced differentiation of promyelocytic HL-60 cells into macrophages. Carcinogenesis involves some modifications in the expression of biomarkers such as cyclooxygenase-2 and matrix metalloprotease-9. The differentiation status could have an impact on the NF-κB signaling pathway that regulates the target genes, given that these target genes expression varies during cell differentiation. We hypothesize that the activation of the NF-κB pathway by PMA can be reverse by (-)-epigallocatechin-gallate (EGCG). Indeed, the up-regulation of downstream genes combined with the down-regulation of IκB expression showed the significant implication of the NF-κB signaling pathway to activate pro-inflammatory and pro-invasive mechanisms linked to carcinogenesis. The same evidence exhibits in the differentiated cells called «macrophages-like». Moreover, the green tea polyphenol, EGCG, shows chemopreventive property since it better inhibited NF-κB signaling in cells treated simultaneously with EGCG and PMA compared to the «macrophages-like». This difference could be due, in part, to the down-regulation of the 67 kDa laminin receptor, known to be the non-integrin membrane receptor for EGCG. All together, our results suggest that the differentiation status of promyelocytic cells is linked to the activation of mechanisms involved in carcinogenesis and metastasis. These phenomena can be prevented by using natural agents such as EGCG. Targeting the specific biomarkers linked to the differentiation status of tumor cells and involved in the disruption of the BBB may help reduce secondary neuroinflammation and enable the advancement of knowledge towards carcinogenesis prevention.

cellules HL-60

inflammation

cyclooxygénase-2

métalloprotéase matricielle (MMP-9)

NF-kB

(-)-épigallocatéchine-3-gallate

HL-60 cells

cyclooxygenase-2

matrix metalloprotease

(-)-epigallocatechin-3-gallate

Avaliação dos produtos finais de glicosilação e o fator nuclear K-B em glandulas lacrimais e superficie ocular de modelos animais de diabetes e envelhecimento / Advanced glycation end-products and Nuclear Factor K-B in lacrimal glands and ocular surface of diabetes and aging animal models

Alves, Monica de Cassia

13 August 2018

Orientador: Eduardo Melani Rocha / Tese (doutorado) - Universidade Estadual de Campinas, Faculdade de Ciencias Medicas / Made available in DSpace on 2018-08-13T17:43:11Z (GMT). No. of bitstreams: 1 Alves_MonicadeCassia_D.pdf: 5666644 bytes, checksum: 2d8f41985c6b80374f8fd6d042fc9ff0 (MD5) Previous issue date: 2006 / Resumo: Este estudo avaliou as possíveis vias comuns na fisiopatogênese da síndrome do olho seco no Diabetes Mellitus (DM) e no envelhecimento, envolvendo o acúmulo dos produtos de glicosilação ("Advanced Glycation End-products" - AGEs), seu receptor RAGE e a ativação do Fator Nuclear-?B (NF-?B) na glândula lacrimal (GL) e alterações do filme lacrimal nessas condições. Modelos animais de DM induzido com estreptozotocina e animais senis (24 meses de vida) foram comparados a animais controle tratados com tampão citrato e adultos jovens (2 meses de vida). Foram avaliadas vias de sinalização, envolvendo AGEs, RAGE e a ativação do NF-?B na GL e alterações no filme lacrimal em ratos Wistar de todos os grupos. A análise do filme lacrimal foi realizada através de medidas de volume de secreção basal e dosagem de citocinas como a Interleucina-1 ß (IL-1 ß) e Fator de Necrose Tumoral - a (TNF- a). A capacidade secretória da GL foi avaliada através de medidas da atividade de peroxidase. Técnicas de "western blot" foram utilizadas para avaliar a expressão e ativação do NF-?B na GL. A expressão de AGE, RAGE e NF-?B na GL e córnea nos grupos estudados, foi avaliada através de microscopia confocal com imunofluorescência. O volume lacrimal foi significativamente menor nos animais diabéticos e senis (P=0,02 e 0,016, respectivamente). Concentrações de IL-1ß e TNF-a na lágrima foram mais altas nos ratos diabéticos e senis do que nos controles e adultos jovens (P=0,007 e 0,02 nos diabéticos e P= 0,007 e P= 0,05 nos senis). A atividade de peroxidase foi significativamente mais baixa no grupo senil (P=0,016), mas não nos experimentos, comparando animais diabéticos e controles (P=0,34). A expressão de AGE, RAGE e NF-?B na GL foi aumentada nos animais diabéticos e senis. O DM e a senilidade induzem alterações estruturais e secretórias significativas na GL e nos tecidos da superfície ocular e associa-se a maior incidência de olho seco. A expressão aumentada de AGE, RAGE e NF-?B na GL sugere a participação desses fatores nas vias de sinalização e subseqüentes alterações inflamatórias relacionadas ao olho seco nessas condições. / Abstract: The present study evaluates the dry eye syndrome related to diabetes and aging through the involvement of the Advanced Glycation End-product (AGEs), the Advanced Glycation End-product Receptor (RAGE) axis and Nuclear Factor-?B (NF-?B) activation in lacrimal gland (LG) and tear film dysfunction in these conditions. To evaluate whether AGE, RAGE and NF-?B signaling in LG are altered in diabetes and aging, streptozotocin-induced diabetic, normoglicaemic, aging (24 month-old) and young adults (2 month-old) male Wistar rats were compared. Tear film alterations and the expression of AGE, RAGE and NF-?B in ocular tissues were evaluated in all considered groups. Tear secretion parameters as basal tear secretion volume, Interleukin-1 ß (IL-1 ß) and Tumor Necrosis Factor- a (TNF- a) levels and LG and peroxidase activity in LG tissue were measured. NF-?B expression and activation was evaluated in LG by western blot. Immunohistochemistry with confocal microscopy was used to assess AGE, RAGE and NF-?B expression in LG of all groups. Tear volume was significantly lower in diabetic and aging rats (P=0.02 and 0.016, respectively). IL-1ß and TNF-a concentrations in tears were higher in diabetic and aging than in control and young rats (P=0.007 and 0.02 in diabetic and P= 0.007 and P= 0.05 in aging). Peroxidase activity was significantly lower in the aging group (P=0.016) but not the assays with diabetic rats (P=0.34). AGE, RAGE and NF-?B expressions were increased in LG of diabetic and aging rats. Diabetes and aging induce significant alterations in rat LG structure and secretion. The higher expression of AGE, RAGE and NF-?B in LG may suggest that these factors are involved in signalling and in subsequent inflammatory alterations related to dry eye related to these conditions. / Doutorado / Clinica Medica / Doutor em Clínica Médica

Aparelho lacrimal

Sindrome do olho seco

Diabetes Mellitus

Fator nuclear K-B

Envelhecimento

Lacrimal apparatus

Dry Eye sindrome

Diabetes

Glycosylation end products

Nuclear factor KB

Aging

Novas funções da proteina AIRE : 1) seu papel na resposta mediada por dectina-1 em fagocitos mononucleares humanos. 2) sua associação com a queratina 17, proteina dos filamentos intermediarios / New roles of AIRE protein : 1) AIRE role in Dection-1 mediated patway in human mononuclear phagocytes and 2) AIRE association with keratin-17, a component of intermediate filaments

Talero, Luis Alberto Pedroza

13 August 2018

Orientador: Antonio Condino Neto / Tese (doutorado) - Universidade Estadual de Campinas, Faculdade de Ciencias Medicas / Made available in DSpace on 2018-08-13T22:05:12Z (GMT). No. of bitstreams: 1 Talero_LuisAlbertoPedroza_D.pdf: 1538530 bytes, checksum: 6dc94ec71cdd6f03d096be015a2b1757 (MD5) Previous issue date: 2009 / Resumo: A Poliendocrinopatia autoimune associada a candidíase e distrofia ectodérmica (APECED) é um síndrome caracterizado pela presença de pelo menos dois sintomas clínicos, endocrinopatia autoimune, sendo que as mais comuns são hipoparatiroidismo, doença de Addison, além de candidíase mucocutânea crônica. É também comum nos pacientes o desenvolvimento de distrofia ectodérmica, como distrofia nas unhas ou alopécia. O APECED é produzido por mutações no gene AIRE, que codifica uma proteína com propriedades reguladoras na transcrição de proteínas ectópicas no timo, o que estaria envolvido na seleção negativa de células T auto-reativas, e conseqüentemente no desenvolvimento da doença autoimune. No entanto a associação da deficiência da proteína AIRE com a suscetibilidade a candidíase ou a distrofia ectodérmica permanecem obscuras. No presente trabalho, investigamos a possibilidade que esta associação esteja envolvida com a expressão e função da proteína AIRE no ambiente extra-tímico. Usando células de sangue periférico de pacientes com mutações no AIRE, e a técnica de SiRNA para silenciar este gene em células de linhagem mielomonocítica THP-1, demonstramos que a proteína AIRE é importante para a resposta via KF-kB dos TLRs e Dectina-1, sendo que AIRE está presente num complexo com Dectina-1, Syk e Card-9, formado após o estímulo com Curdlan. Além disso demonstramos que a formação deste complexo pode acontecer no citoplasma ou membrana citoplasmática, uma vez que após este estímulo, a proteína AIRE é exportada do núcleo permanecendo temporariamente na membrana. Finalmente usando a técnica de espectroscopia de massa e microscopia confocal, mostramos que AIRE interage com a proteína Queratina 17, tanto em células THP-1 como em células HaCaT (linhagem de queratinócitos), quando as células entram num estágio de espraiamento e migração. Assim, a presença da proteína AIRE na via de sinalização da Dectina-1, pode estar relacionada com a susceptibilidade a infecções crônicas por C. albicans observada nestes pacientes. A resposta imune via Dectina-1 é importante na resposta a este fungo e defeitos na molécula CARD9 e Dectina-1 podem estar associados a Candidíase mucocutânea crônica. Por outro lado, a descrição da associação de AIRE com K17 pode ser relevante, já que pacientes com mutações no gene que codifica para a proteína K17 desenvolvem uma doença chamada paquioníquia congênita, caracterizada por distrofia das unhas e alopécia, características clínicas observadas também nos pacientes com APECED. Deste modo, neste trabalho apresentamos evidências que apontam para um novo papel funcional da proteína AIRE no ambiente extratímico, que poderia explicar em parte algumas características clínicas dos pacientes com APECED, como a elevada suscetibilidade a infecções por C. albicans, e a distrofia ectodérmica / Abstract: The autoimmune polyendocrinopathy candidiasis and ectodermal dystrophy (APECED) is characterized by the presence of two from three major clinical symptoms: Addison's disease, and/or hypoparathyroidism, and/or chronic mucocutaneous candidiasis. These patients develop also ectodermal dystrophies like nail dystrophy and alopecia. APECED is caused by mutations in the autoimmune regulator gene (AIRE). This gene encodes a protein with DNA binding capacity that can transcriptionally modulate ectopic peripheral tissue antigen (PTA) expression in the thymus, facilitating T cell negative selection. Defects in AIRE may be related with the development of multipleendocrine failure of autoimmune origin in patients with APECED. In spite of this, the role of AIRE deficiency in the C. albicans susceptibility or ectodermal dystrophy, common features in APECED patients, remains to be elucidated. In the present work we explored the hypothesis that candidiasis and ectodermal dystrophy are associated with the extra-thymic role of AIRE. For this we used peripheral blood mononuclear cells from APECED patients, and also THP-1 cells treated with SiRNA for AIRE gene to obtain AIRE deficient cells. We demonstrated that AIRE is required for Dectin-1- and TLR-ligand-induced inflammatory response and complexes with Dectin-1, Syk, and CARD9 after Curdlan stimulation. In addition, we showed that this complex formation takes place outside the nucleus, once that after Curdlan stimulation AIRE seems to be exported to the cytoplasm and transiently locate at the cytoplasmic membrane. Finally using mass spectra and confocal microscopy, we showed an interaction between AIRE and the intermediate filament protein Keratin-17, in both THP-1 cells and the keratinocyte cell line HaCaT. Therefore, the presence of AIRE protein in Dectin-1 pathway seems to be important on the C. albicans response, and the absence of this protein could be a risk factor important for developing candidiasis, commonly observed in APECED patients. This observation is supported by the fact that Dectin-1 is important for C albicans response, and also the recently description of mutations in Dectin-1 and CARD9 and its association with chronic mucocutaneous candidiasis. On the other hand, the description of AIRE and K17 association is important, since patients with defects on K17 gene develop congenital pachyonychia, a disease characterized by nail dystrophy and alopecia, also observed in APECED patients. Thus we provided evidence for a new role of AIRE protein in the extrathymic environment, which in may explain, at least in part, some of the common clinical features other than autoimmunity, observed in APECED patients / Doutorado / Saude da Criança e do Adolescente / Doutor em Saude da Criança e do Adolescente

Proteina AIRE

APECED, proteina humana

Dectin-1

NF-kappa B

Candidíase

Imunidade natural

Queratina-17

Filamentos intermediarios

AIREprotein

APECED protein, human

Dectin-1

NF-kB

Candidiasis

Immunity, Natural

Keratin-17

Intermediate filaments

Rôles de TRIM5 et Atg5 dans la réponse immune innée de cellules infectées par le VIH-1

Khalfi, Soumia

January 2020

No description available.

UQTR Biologie cellulaire et moléculaire

Activité antirétrovirale

Activité pro-inflammatoire

AP-1

Autophagie

ATG5

Cellules infectées

CRISPR

Flavivirus

IFN-bêta

Immunité innée

NF-kB

p62

Réponse immune innée

Restriction

SiDA

TRIM5

Trim5a

Trim5alpha

VIH-1

Virus de l'immunodéficience humaine

Grafické intro 64kB s použitím OpenGL / Graphics Intro 64kB Using OpenGL

Burkot, Martin

January 2011

This thesis deals with the creation of minimal graphics intro. Intro size is not extending 64kB. The base of the intro is procedurally generated terrain supplemented with procedural vegetation and texture representing clouds. It also has terrain texture and imported 3D models. As background music is music playing.