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Showing 1 to 10 of 10 (0.049 seconds)Spelling suggestions: "subject:"death receptors"" "subject:"heath receptors""
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Charakterizace TRAILem indukované, receptor-specifické signalizace v nádorových buňkách. / Charakterizace TRAILem indukované, receptor-specifické signalizace v nádorových buňkách.Peterka, Martin January 2013 (has links)
TNF-related apoptosis-inducing ligand (TRAIL) is a member of TNF family expressed mainly by hematopoietic cells. TRAIL brought significant attention mainly for its ability to trigger apoptosis in a number of cancer cells. In addition to apoptosis, TRAIL can induce several other signaling pathways such as activation of MAP kinases or canonical NF-B signaling. Human TRAIL can bind to five receptors but only two of them (death receptors TRAIL-R1/DR4 and TRAIL-R2/DR5) can trigger TRAIL-mediated apoptotic and non-apoptotic signaling in target cells. Both receptors are ubiquitously expressed on normal and cancer cells, but the relative contribution of DR4 and DR5 to TRAIL-induced signaling is not well known. Using DR4/DR5-specific variants of TRAIL, we examined how individual receptor contributes to the induction of apoptosis and NF-B, JNK, p38, ERK1/2 and TAK1 signaling pathways in selected colorectal cells. We found that in DLD-1 cells, apoptosis and activation of JNKs are mainly mediated by DR4-selective ligand. In TRAIL-resistant HT-29 cells, we show that though DISC formation and activation of caspase-8 proceeds mainly via DR4-specific signaling, activation of NF-B pathway is mainly triggered by DR5 selective ligand. In other cells and analyzed signaling pathways both receptor-specific ligands triggered very...
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Xenopus p75 neurotrophin receptor : molecular cloning and functional analysis during the early phase of cell death in developing retina /Hutson, Lara Diane. January 1998 (has links)
Thesis (Ph. D.)--University of Washington, 1998. / Vita. Includes bibliographical references (leaves [76]-93).
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La fluoxétine, un antidépresseur de la famille des Inhibiteurs Sélectifs de la Recapture de la Sérotonine : effets apoptotiques et mécanismes d’action dans les lymphocytes humains / Fluoxetine, a Selective Serotonin Reuptake Inhibitor antidepressant : apoptotic effects and signalling in human lymphocytesCharles, Emilie 13 December 2012 (has links)
Les antidépresseurs de type Inhibiteur Sélectif de la Recapture de la Sérotonine (SSRI pour Selective Serotonin Reuptake Inhibitor), dont fait partie la fluoxétine (Prozac), ont été décrits comme capables de déclencher l'apoptose de cellules tumorales in vitro et in vivo, suggérant une potentielle utilisation de ces molécules pour le traitement des cancers. Cependant, leur mécanisme apoptotique n’a pas été élucidé à ce jour. Nous avons donc entrepris de déterminer les étapes de l'apoptose induite par la fluoxétine et les SSRI, en choisissant comme modèle d'étude des lignées cellulaires de lymphomes non-Hodgkiniens agressifs. Nous avons identifié plusieurs étapes de la signalisation apoptotique de la fluoxétine et des SSRI. Ainsi, via une inhibition de la chaîne respiratoire, la fluoxétine induit la production d'espèces réactives de l'oxygène conduisant à la surexpression des récepteurs de mort DR4 et DR5 ; la fluoxétine induit également l'activation de la caspase-8. DR4 et DR5 sont très probablement la cause de l'apoptose induite par la fluoxétine, de façon indépendante de leur ligand, TRAIL (TNF-Related Apoptosis-Inducing Ligand). Partant du constat que l'utilisation de TRAIL comme antitumoral pour le traitement des lymphomes présente des résultats prometteurs mais encore insuffisants, nous avons envisagé que la fluoxétine puisse augmenter l’apoptose induite par TRAIL dans ce type de tumeurs. Nous montrons en effet qu'une association de la fluoxétine avec TRAIL conduit à une augmentation de l'action apoptotique de TRAIL dans les lignées de lymphomes non-Hodgkiniens agressifs. De plus, nos résultats montrent que la fluoxétine induit la mort cellulaire d'une façon indépendante de la caspase-8. Cet effet semble trouver son origine dans une surcharge en calcium de la mitochondrie, alimentée par une stimulation maintenue de l'entrée de calcium par les canaux CRAC (Calcium Release Activated Calcium). En conclusion, les éléments de la signalisation calcique et apoptotique de la fluoxétine et des SSRI que nous avons identifiés encouragent leur utilisation en thérapie, et notamment dans le cadre d'associations avec TRAIL et d'autres molécules pour permettre une augmentation de l'apoptose des cellules tumorales, voire des cellules résistantes à l'apoptose induite par TRAIL. / Selective Serotonin Reuptake Inhibitor (SSRI) antidepressants, such as fluoxetine (Prozac), have been shown to induce apoptosis in cancer cells in vitro and in vivo, suggesting a potential use for cancer treatment. However, their apoptotic mechanism has remained undetermined until now. Therefore, we have undertaken the determination of fluoxetine- and SSRIs-induced apoptotic signalling, our study model being aggressive Non-Hodgkin's Lymphoma (NHL) cell lines. We have identified several steps of the apoptotic signalling of fluoxetine and the SSRIs. Thus, via an inhibition of the respiratory chain, fluoxetine induces a reactive oxygen species production leading to the overexpression of the death receptors DR4 and DR5; fluoxetine also induces caspase-8 activation. DR4 and DR5 are probably the cause of fluoxetine-induced apoptosis, independently of their ligand TRAIL (TNF-Related Apoptosis-Inducing Ligand). Knowing that TRAIL as an antitumoral agent for lymphoma treatment has shown promising but insufficient results, we have hypothesized that fluoxetine could increase TRAIL-induced apoptosis in these tumors. Indeed, we show that fluoxetine in association with TRAIL leads to an increase in TRAIL-induced apoptosis in aggressive NHL cell lines. Furthermore, our results show that fluoxetine induces cell death in a caspase-8–independent manner. This effect seems to originate from a mitochondrial calcium overload fueled by a sustained calcium entry from the CRAC (Calcium Release Activated Calcium) channels. In conclusion, the calcium pathway and the apoptotic steps of the fluoxetine's and the SSRIs' signalling that we have delineated encourage their use in therapy, especially in association with TRAIL and other molecules in order to enable an increase in cancer cells' apoptosis, or even in cancer cells which are resistant to TRAIL-induced apoptosis.
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Role of TRAIL-receptors in apoptosis and nonapoptotic signaling in cancer cells populations undergoing fractional killing / Décryptage du rôle de l'activation des récepteurs de TRAIL dans l'induction de l'apoptose ou de la signalisation de la survie au sein d'une même population de cellules cancéreusesShlyakhtina, Yelyzaveta 22 September 2016 (has links)
TRAIL (Tumor necrosis factor-Related Apoptosis-Inducing Ligand) induit l’apoptose des cellules cancéreuses de manière sélective, tout en épargnant les cellules saines. TRAIL peut aussi activer des voies de signalisation de survie cellulaire dans des cellules cancéreuses résistantes à l’induction de la mort programmée après traitement. Les cellules cancéreuses que nous avons étudiées sont caractérisées par un phénotype de mort cellulaire fractionnée en réponse à TRAIL, c’est-à-dire que seule une fraction de la population meurt en présence de TRAIL, alors que l’autre fraction active la survie cellulaire. Lors de notre étude nous avons montré que les récepteurs de TRAIL jouent un rôle particulièrement important dans l’engagement de ces cellules vers l’une ou l’autre de ces voies. De telles recherches permettront de mieux appréhender la complexité de la signalisation TRAIL-dépendante, et de proposer des thérapies combinées qui réduiront la progression tumorale induite par TRAIL. / Tumor necrosis factor-Related Apoptosis-Inducing Ligand (TRAIL) gives a promise for cancer selective therapy as it exclusively induces apoptosis in tumor cells while sparing normal tissues. TRAIL also activates pro-survival pathways in cancer cells resistant to TRAIL-induced cell death. In this study we used clonal populations of cancer cells that respond in fractional killing upon TRAIL treatment: only a fraction of a clonal cancer cell population dies while another survives, activates non-apoptotic cascades and proliferates. We found that TRAIL receptors play an important role in the bifurcation of TRAIL signaling in populations of cancer cells that respond in fractional killing upon TRAIL challenge. These results will provide insights for evaluating whether combined therapies targeting components promoting the activation of pro-survival signaling would allow the use of rhTRAIL/DR5 agonistic antibodies to activate TRAIL-mediated killing while avoiding TRAIL-induced tumor progression.
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Charakterizace vlivu senescence na indukci a regulaci smrti nádorových buněk / Charakterizace vlivu senescence na indukci a regulaci smrti nádorových buněkNováková, Gita January 2014 (has links)
4 Abstract Senescence is a specific cell state distinquished by cessation of cell division and proliferation and changes in gene expression. Normal cells enter senescence after distinct number of cell divisions or in case of an unrepairable damage. Senescence in cancer cells can be induced by subliminal stress as sublethal treatment with certain drugs. Senescent cancer cells persist in the tissue and may secrete a number of factors and nutrients affecting surrounding cells. Senescence can thus change the response of cancer cells to various apoptogens during cancer therapy. In this study, we focused on the elucidation of presumed differences between normal proliferating and senescent cancer cells in their response to selected apoptogens. Implementing bromodeoxyuridine (BrdU)-mediated replication stress in cancer cells derived from pancreatic (PANC-1) or mesothelioma (H28) tumors, we efficiently forced these cells to acquire senescent phenotype. We document that these senescent cells gain higher resistance to combined TRAIL and homoharringtonine (HHT) treatment and enhance sensitivity to other apoptogens such as FasL, camptothecin and mVES. These cells also showed increased expression of anti-apoptotic protein c-FLIP in senescent cells and changes in the expression of some Bcl-2 family proteins....
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Controle da expressão de TRAIL, OSM, FAIM e NIPA pelo oncogene bcr-abl. / bcr-abl regulation of TRAIL, OSM, FAIM and NIPA expression.Leroy, Janine Marie Gisele 03 July 2008 (has links)
A leucemia mielóide crônica (LMC) é uma doença mieloproliferativa e sua patogênese está associada à expressão de um neogene, bcr-abl, que codifica uma proteína tirosina quinase Bcr-Abl. Esse trabalho tem como objetivos o estudo dos mecanismos envolvidos na resistência à morte das células Bcr-Abl positivas e a identificação de alterações gênicas nessas células. Dados de expressão gênica global obtidos por \"microarray\" mostraram uma superexpressão nas células HL-60.Bcr-Abl com relação a HL-60 dos genes faim e nipa, que foi confirmada por qRT-PCR em diferentes linhagens celulares Bcr-Abl positivas. Já os genes de trail e osm, apresentaram uma diminuição significativa em HL-60.Bcr-Abl, que foi confirmada para trail, porém osm não teve seu resultado validado. A avaliação da expressão dos genes em células de pacientes portadores de LMC, em diferentes fases da doença também foi estudada. Com esses resultados, o presente estudo visa a melhor compreensão de como alterações na expressão desses genes contribuem na fisiopatologia da LMC. / Chronic myelogenous leukemia (CML) is a stem cell disease characterized by the presence of the Bcr-Abl oncoprotein, which is the cause of the malignant transformation and the extreme resistance to apoptosis displayed by CML patients. Our aim was to analyze the alteration in global gene expression in Bcr-Abl expressing cells. Data obtained from microarray analysis showed significant up-regulation of nipa and faim in HL60.Bcr-Abl and down-regulation of osm and trail. These results were further confirmed by Real-Time PCR to nipa, faim and trail, but not for osm expression in HL-60.Bcr-Abl cells. To evaluate the potential of some of the modified genes as therapeutic targets or prognostic markers for CML, we also analyzed the expression of these genes in samples from CML patients.
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Controle da expressão de TRAIL, OSM, FAIM e NIPA pelo oncogene bcr-abl. / bcr-abl regulation of TRAIL, OSM, FAIM and NIPA expression.Janine Marie Gisele Leroy 03 July 2008 (has links)
A leucemia mielóide crônica (LMC) é uma doença mieloproliferativa e sua patogênese está associada à expressão de um neogene, bcr-abl, que codifica uma proteína tirosina quinase Bcr-Abl. Esse trabalho tem como objetivos o estudo dos mecanismos envolvidos na resistência à morte das células Bcr-Abl positivas e a identificação de alterações gênicas nessas células. Dados de expressão gênica global obtidos por \"microarray\" mostraram uma superexpressão nas células HL-60.Bcr-Abl com relação a HL-60 dos genes faim e nipa, que foi confirmada por qRT-PCR em diferentes linhagens celulares Bcr-Abl positivas. Já os genes de trail e osm, apresentaram uma diminuição significativa em HL-60.Bcr-Abl, que foi confirmada para trail, porém osm não teve seu resultado validado. A avaliação da expressão dos genes em células de pacientes portadores de LMC, em diferentes fases da doença também foi estudada. Com esses resultados, o presente estudo visa a melhor compreensão de como alterações na expressão desses genes contribuem na fisiopatologia da LMC. / Chronic myelogenous leukemia (CML) is a stem cell disease characterized by the presence of the Bcr-Abl oncoprotein, which is the cause of the malignant transformation and the extreme resistance to apoptosis displayed by CML patients. Our aim was to analyze the alteration in global gene expression in Bcr-Abl expressing cells. Data obtained from microarray analysis showed significant up-regulation of nipa and faim in HL60.Bcr-Abl and down-regulation of osm and trail. These results were further confirmed by Real-Time PCR to nipa, faim and trail, but not for osm expression in HL-60.Bcr-Abl cells. To evaluate the potential of some of the modified genes as therapeutic targets or prognostic markers for CML, we also analyzed the expression of these genes in samples from CML patients.
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Étude du récepteur CD95 et de son rôle pro-inflammatoire dans le lupus / Study of the CD95 receptor and its proinflammatory role in lupusSanséau, Doriane 30 September 2015 (has links)
Le récepteur de mort CD95 participe à de nombreuses fonctions physiologiques en transmettant des signaux apoptotiques. Son ligand membranaire, CD95L, est principalement exprimé à la surface des lymphocytes et contrôle ainsi l’homéostasie cellulaire et l’élimination des cellules infectées ou transformées. Certaines situations pathologiques conduisent à une expression ectopique du CD95L par d’autres types cellulaires,associé à son clivage par des métalloprotéases (cl-CD95L). La forme soluble ainsi libérée perd sa capacité à transmettre l’apoptose mais déclenche l’activation de voies non-apoptotiques induisant l’inflammation dans des maladies inflammatoires chroniques comme le lupus érythémateux systémique (LES) ou encore les formes métastatiques du cancer du sein. Dans ces deux pathologies, de fortes quantités de cl-CD95L sont détectées dans le sérum de ces patients et ont été associés à la progression des pathologies. Dans le LES, nous établissons que cl-CD95L contribue au processus inflammatoireen favorisant la transmigration endothéliale des lymphocytes Th17. Cette migration cellulaire dépendante de CD95 nécessitele recrutement de la PLCγ1 sur le domaine juxta-membranaire de CD95 qui induitl’activation du signal calcique. Pour identifier d’autres partenaires moléculaires de CD95, une analyse protéomique a été réalisée et a permis d’identifier une association entre CD95 et la machinerie traductionnelle. Cette interaction nécessite le recrutement d’eIF4A1 au niveau du domaine juxta-membranaire de CD95. Nous avons par ailleurs montré que dans des lignées cancéreuses mammaires, eIF4A1 participe à la traduction de certaines protéines comme la sérine-thréonine kinase Akt pour faciliter l’activation de la voie de signalisation PI3K et la migration cellulaire induite par CD95. Cette étude a donc mis en évidence l’implication d’un nouveau domaine de CD95 dans l’induction des signaux non-apoptotiques. Ce domaine juxta-membranaire a été nommé CID pour « calcium inducing domain ». De plus, ce domaine fusionné à un peptide perméant provenant de la protéine TAT appelé TAT-CIDa montré son efficacité pour inhiber la migration lymphocytaire chez les souris lupiques et offre de nouvelles perspectives pour le développement de traitements améliorants les symptômes inflammatoires du LES. / The death ligand CD95L, mainly expressed by immune cells, contributes to the elimination ofinfected and transformed cells. In pathological contexts, CD95L can be expressed by others cell types such as endothelial cells.CD95L can be cleaved by metalloproteases to generate a soluble CD95L (cl-CD95L) failing to trigger the apoptotic signaling pathwaybutinducing non-pro-apoptotic signaling pathways. cl-CD95L promotes inflammation in chronic inflammatory disorders such as systemic lupus erythematosus (SLE) and increases risks of metastatic dissemination in breast cancer patients. In SLE patients, we established that high amounts of cl-CD95L fuels inflammation by promoting endothelial transmigration of activated Th17 cells. This CD95-drivencell migration requires PLCγ1 recruitment by CD95 and the subsequentimplementation of the calcium signal. To identify in an exhaustive fashion, all molecular partners of CD95, a global proteomic analysis was undertaken. This TAP-Tag approach highlighted a strong association between the translational machinery and CD95. This analysis was confirmed by a two-hybrid approach revealingthat the translation initiation factor eIF4A1 directly interactedwith CD95.In breast cancer cells, we established that eIF4A1 was instrumental in the translation of certain genes such as Akt contributing to the implementation of the CD95-mediated PI3K signaling pathway and cell migration. In this study, we identifiedthe CD95 domaininvolved in the induction of the non-apoptotic signaling pathway. This domain was named CID for “calcium inducing domain”.Moreover, wegenerated a therapeutic molecule consisting of theCID fused to the cationic cell-penetrating HIV TAT domain. TAT-CID prevented the accumulation of Th17 cells in inflamed organs of lupus-prone mice and could turn out to be an original therapeutic molecule to alleviate clinical symptoms in SLE patients.
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Avaliação da expressão de genes e proteínas anti- e pró-apoptóticos em pacientes com diabetes mellitus tipo 1 e esclerose múltipla submetidos ao transplante autólogo de células-tronco hematopoéticas / Evaluation of anti and proapoptotic gene and protein expression in type 1 diabetes mellitus and multiple sclerosis patients submitted to autologous hematopoietic stem cell transplantationOliveira, Gislane Lelis Vilela de 17 October 2008 (has links)
O diabetes mellitus tipo 1 (DM-1) e a esclerose múltipla (EM) são doenças auto-imunes órgão-específicas, inflamatórias, mediadas por células T e B auto-reativas e caracterizadas pela destruição seletiva de células b pancreáticas produtoras de insulina e do sistema nervoso central, respectivamente. Acredita-se que a desregulação da expressão de genes reguladores da maquinaria apoptótica possa contribuir para o desenvolvimento da auto-imunidade, visto que algumas dessas moléculas participam nos processos de tolerância central e periférica de linfócitos auto-reativos. O objetivo deste projeto foi analisar a expressão de moléculas reguladoras das vias intrínseca, extrínseca e da Família de proteínas inibidoras da apoptose (IAP) em 33 indivíduos saudáveis, 15 pacientes com DM-1 e 18 com EM submetidos à terapia de imunossupressão em altas doses seguida do transplante autólogo de células-tronco hematopoéticas (IAD/TACTH). As células mononucleares (CMN) foram isoladas do sangue periférico dos controles e de pacientes nos períodos pré-mobilização (pré-mob), pré-condicionamento (pré-cond), D+180, D+360, D+540 e D+720 pós-transplante. As CMN foram utilizadas para extração de RNA, síntese de cDNA, quantificação da expressão por PCR em tempo real dos genes a1, bcl-2, bcl-w, bcl-xL, mcl-1, bad, bak, bax, bid, bik, bim, bok, noxa, fas, fasL, c-FLIPL, cIAP-1 e cIAP-2 e protéica de Bcl-2, Bcl-xL, Bak, Bim e c-FLIPL por western-blotting. Os resultados de expressão gênica foram representados por unidades relativas de expressão em medianas nas diferentes amostras. Os pacientes com DM-1 apresentaram diminuição da expressão dos genes anti-apoptóticos bcl-2 (mediana: 0,98; p=0,04), bcl-w (0,08; p=0,04), mcl-1 (1254; p=0,03) e cIAP-1 (1,24; p=0,003) nas CMN dos pacientes no período pré-mob em relação aos indivíduos saudáveis (medianas: bcl-2: 7,58; bcl-w: 0,52; mcl-1: 1659; cIAP-1: 14,5), enquanto a expressão de cIAP-2 (60,8; p=0,0005) estava aumentada em relação aos controles (23,3). Foi observada redução significativa na expressão dos genes pró-apoptóticos bad (0,002; p<0,0001), bax (0,01; p=0,002) e fasL (1,66; p=0,001) no período pré-mob comparada aos controles sadios (bad: 0,23; bax: 2,79; fasL: 3,56). Os níveis de RNAm de bid (0,10; p=0,001) e bok (0,72; p=0,006) estavam elevados no pré-mob em relação ao grupo controle (bid: 0,004; bok: 0,31). As moléculas bcl-2, bcl-w, bcl-xL, mcl-1, bad, bax, bok, fasL e cIAP-1 atingiram níveis de RNAm similares aos controles após o TACTH. Foi verificado que a expressão de bcl-w, cIAP-1 e noxa estava maior nos pacientes com DM-1 em remissão quando comparados àqueles em recaída. A diminuição da expressão de a1, bcl-2 e bcl-w e o aumento de fas e noxa correlacionaram-se às porcentagens de hemoglobina glicosilada, concentração de auto-anticorpos GAD65, e aos níveis séricos de peptídeo-C após o transplante. Os pacientes com EM mostraram uma expressão reduzida dos genes anti-apoptóticos bcl-w (0,11; p=0,02) e cIAP-1 (1,87; p=0,04) no pré-mob comparada aos valores dos controles (bcl-w: 0,27; cIAP-1: 7,75) e maior expressão dos genes a1 (90,8; p=0,001) e cIAP-2 (58,8; p=0,009) em relação aos controles (a1: 12,7; cIAP-2: 22,3). As moléculas pró-apoptóticas bad (0,007; p=0,01) e bax (0,0007; p=0,004) mostraram menor expressão nas CMN no período pré-mob do que nos controles (bad: 0,27; bax: 1,24). Os genes bid (20,7; p=0,004), bik (0,84; p=0,02) e bok (1,77; p=0,0001) possuíam maior expressão no período pré-mob em relação aos indivíduos sadios (bid: 2,64; bik: 0,33; bok: 0,26). Não foram observadas diferenças significativas na expressão das moléculas da via extrínseca da apoptose nos pacientes com EM (p>0,05) nos períodos avaliados. Os valores de expressão de bcl-w, bak, bax, bik, bok e cIAP-1 atingiram níveis semelhantes aos controles após o transplante. A expressão dos genes bcl-2, cIAP-1, bad e bax estava maior nos pacientes em remissão da EM quando comparados àqueles em progressão neurológica. O aumento da expressão dos genes pró-apoptóticos bax, bak e bimEL correlacionou-se inversamente aos valores de EDSS dos pacientes com EM após o TACTH. Os resultados de expressão protéica foram equivalentes aos de expressão gênica nas duas doenças, com exceção dos dados das proteínas Bcl-2 e Bim. Em conjunto, os resultados demonstraram a desregulação da expressão de várias moléculas anti- e pró-apoptóticas nas CMN dos pacientes com DM-1 e EM. Esses achados sugerem a associação de alterações nos processos de apoptose celular com o surgimento e persistência de células auto-reativas no DM-1 e EM. Os dados indicam que essas alterações, principalmente a diminuição da expressão de moléculas pró-apoptóticas, como bak e bax, possam contribuir para a patogênese do DM-1 e EM. Além disso, a terapia de IAD/TACTH foi capaz de modular a expressão da maioria dos genes anormalmente expressos nas CMN dos pacientes com DM-1 e EM, já que esses atingiram níveis de expressão similares ao grupo controle após o transplante. Esta normalização da expressão de vários genes analisados correlacionou-se com a remissão clínica da doença na maioria dos pacientes / Type 1 diabetes mellitus (T1DM) and multiple sclerosis (MS) are inflammatory, organ-specific autoimmune diseases characterized by selective destruction of insulin-producing pancreatic -cells and central nervous system, respectively, by autoreactive B and T cells. Deregulation of apoptotic machinery is supposed to contribute to self-tolerance breakdown and autoimmune diseases pathogenesis, since apoptotic molecules have an important role in B and T lymphocytes central and peripheral tolerance mechanisms. The aim of this study was to evaluate the expression of pro and anti-apoptotic molecules from intrinsic and extrinsic apoptotic pathways and IAP Family members in 33 healthy individuals, 15 T1DM and 18 MS patients submitted to high-dose immunossupression therapy followed by autologous hematopoietic stem cell transplantation (HDI/AHSCT). Peripheral blood mononuclear cells (PBMC) were isolated from controls and patients at pre-mobilization (pre-mob), pre-conditioning (pre-cond), D+180, D+360, D+540 and D+720 post-transplantation. PBMC were used for RNA extraction, cDNA synthesis, gene quantification of a1, bcl-2, bcl-w, bcl-xL, bad, bak, bax, bid, bik, bimEL, bok, noxa, fas, fasL, c-FLIPL, cIAP-1 and cIAP-2 by Real Time PCR and Bcl-2, Bcl-xL, Bak, BimEL and c-FLIPL proteins detection by western-blotting. Results are expressed as median of relative expression units. Results from T1DM patients indicated that antiapoptotic molecules bcl-2 (median: 0,98; p=0,04), bcl-w (0,08; p=0,04), mcl-1 (1254; p=0,03) and cIAP-1 (1,24; p=0,003) were downregulated at pre-mob compared with healthy controls (medians bcl-2: 7,58; bcl-w: 0,52; mcl-1: 1659; cIAP-1: 14,5), while cIAP-2 (60,8; p=0,0005) gene expression was upregulated compared to healthy controls (23,3). We observed a significant decrease in proapoptotic bad (0,002; p<0,0001), bax (0,01; p=0,002) and fasL (1,66; p=0,001) genes expression in patients PBMC at pre-mob period compared to healthy subjects (bad: 0,23; bax: 2,79; fasL: 3,56). mRNA levels of bid (0.10; p=0.001) and bok (0.72; p=0.006) were elevated at pre-mob period when compared to control group (bid: 0.004; bok: 0.31). The bcl-2, bcl-w, bcl-xL, mcl-1, bad, bak, bax, bok, fasL and cIAP-1 mRNA levels reached controls levels after HDI/AHSCT. We observed that bcl-w, cIAP-1 and noxa gene expression were increased in T1DM patients in remission when compared to relapsed patients. The decreased antiapoptotic gene expression and increased in proapoptotic molecules correlated with decreased glicosilated hemoglobin percentages (Hb A1C) and anti-GAD65 antibodies and increased peptide-C levels. Results from MS patients showed decreased bcl-w (0,11; p=0,02) and cIAP-1 gene expression (1,87; p=0,04) in patients PBMC at pre-mob period compared to healthy controls (bcl-w: 0,27; cIAP-1: 7,75) and increased expression of a1 (90,8; p=0,001) and cIAP-2 (58,8; p=0,009) compared to controls (a1: 12,7; cIAP-2: 22,3). Proapoptotic molecules bad (0.007; p=0.01) and bax (0.0007; p=0.004) showed decreased gene expression at pre-mob compared to control group (bad: 0.27; bax: 1.24). bid (20.7; p=0.004), bik (0.84; p=0.01) and bok genes (1.77; p=0.0001) showed increased expression at pre-mob compared to healthy controls (bid: 2.64; bik: 0.33; bok: 0.26). Significant differences were not observed in the expression of the extrinsic pathway genes in pre-mob and healthy controls samples (p>0.05). bcl-w, bak, bax, bik, bok and cIAP-1 expression values reached healthy control values after transplantation. We observed that bcl-2, cIAP-1, bad and bax gene expression was increased in MS patients in disease remission when compared to patients with neurologic progression. Significant correlation of increased proapoptotic genes expression with decreased EDSS values in MS patients after HDI/AHSCT was observed. Results of protein quantification of apoptotic molecules in PBMC of T1DM and MS patients were similar to the gene expression results of these molecules, except for Bcl-2 and Bim proteins. Taken together, these data indicate a deregulated expression of anti- and proapoptotic genes in T1DM and MS patients PBMC. These data suggest an association of deregulated apoptosis with emergence and maintenance of autoreactive lymphocytes in analyzed patients. Based on these results, we suggest that this altered gene expression profile, mainly the decreased proapoptotic genes expression, as bak and bax, may contribute to T1DM and MS pathogenesis. Furthermore, we showed that the HDI/AHSCT therapy was able to modulate and normalize the expression of most genes abnormally expressed in T1DM and MS patients at pre-transplant period. Many analyzed genes achieved expression levels similar to healthy controls. The normalization of the expression of many evaluated genes correlated to disease remission in the majority of the patients.
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Avaliação da expressão de genes e proteínas anti- e pró-apoptóticos em pacientes com diabetes mellitus tipo 1 e esclerose múltipla submetidos ao transplante autólogo de células-tronco hematopoéticas / Evaluation of anti and proapoptotic gene and protein expression in type 1 diabetes mellitus and multiple sclerosis patients submitted to autologous hematopoietic stem cell transplantationGislane Lelis Vilela de Oliveira 17 October 2008 (has links)
O diabetes mellitus tipo 1 (DM-1) e a esclerose múltipla (EM) são doenças auto-imunes órgão-específicas, inflamatórias, mediadas por células T e B auto-reativas e caracterizadas pela destruição seletiva de células b pancreáticas produtoras de insulina e do sistema nervoso central, respectivamente. Acredita-se que a desregulação da expressão de genes reguladores da maquinaria apoptótica possa contribuir para o desenvolvimento da auto-imunidade, visto que algumas dessas moléculas participam nos processos de tolerância central e periférica de linfócitos auto-reativos. O objetivo deste projeto foi analisar a expressão de moléculas reguladoras das vias intrínseca, extrínseca e da Família de proteínas inibidoras da apoptose (IAP) em 33 indivíduos saudáveis, 15 pacientes com DM-1 e 18 com EM submetidos à terapia de imunossupressão em altas doses seguida do transplante autólogo de células-tronco hematopoéticas (IAD/TACTH). As células mononucleares (CMN) foram isoladas do sangue periférico dos controles e de pacientes nos períodos pré-mobilização (pré-mob), pré-condicionamento (pré-cond), D+180, D+360, D+540 e D+720 pós-transplante. As CMN foram utilizadas para extração de RNA, síntese de cDNA, quantificação da expressão por PCR em tempo real dos genes a1, bcl-2, bcl-w, bcl-xL, mcl-1, bad, bak, bax, bid, bik, bim, bok, noxa, fas, fasL, c-FLIPL, cIAP-1 e cIAP-2 e protéica de Bcl-2, Bcl-xL, Bak, Bim e c-FLIPL por western-blotting. Os resultados de expressão gênica foram representados por unidades relativas de expressão em medianas nas diferentes amostras. Os pacientes com DM-1 apresentaram diminuição da expressão dos genes anti-apoptóticos bcl-2 (mediana: 0,98; p=0,04), bcl-w (0,08; p=0,04), mcl-1 (1254; p=0,03) e cIAP-1 (1,24; p=0,003) nas CMN dos pacientes no período pré-mob em relação aos indivíduos saudáveis (medianas: bcl-2: 7,58; bcl-w: 0,52; mcl-1: 1659; cIAP-1: 14,5), enquanto a expressão de cIAP-2 (60,8; p=0,0005) estava aumentada em relação aos controles (23,3). Foi observada redução significativa na expressão dos genes pró-apoptóticos bad (0,002; p<0,0001), bax (0,01; p=0,002) e fasL (1,66; p=0,001) no período pré-mob comparada aos controles sadios (bad: 0,23; bax: 2,79; fasL: 3,56). Os níveis de RNAm de bid (0,10; p=0,001) e bok (0,72; p=0,006) estavam elevados no pré-mob em relação ao grupo controle (bid: 0,004; bok: 0,31). As moléculas bcl-2, bcl-w, bcl-xL, mcl-1, bad, bax, bok, fasL e cIAP-1 atingiram níveis de RNAm similares aos controles após o TACTH. Foi verificado que a expressão de bcl-w, cIAP-1 e noxa estava maior nos pacientes com DM-1 em remissão quando comparados àqueles em recaída. A diminuição da expressão de a1, bcl-2 e bcl-w e o aumento de fas e noxa correlacionaram-se às porcentagens de hemoglobina glicosilada, concentração de auto-anticorpos GAD65, e aos níveis séricos de peptídeo-C após o transplante. Os pacientes com EM mostraram uma expressão reduzida dos genes anti-apoptóticos bcl-w (0,11; p=0,02) e cIAP-1 (1,87; p=0,04) no pré-mob comparada aos valores dos controles (bcl-w: 0,27; cIAP-1: 7,75) e maior expressão dos genes a1 (90,8; p=0,001) e cIAP-2 (58,8; p=0,009) em relação aos controles (a1: 12,7; cIAP-2: 22,3). As moléculas pró-apoptóticas bad (0,007; p=0,01) e bax (0,0007; p=0,004) mostraram menor expressão nas CMN no período pré-mob do que nos controles (bad: 0,27; bax: 1,24). Os genes bid (20,7; p=0,004), bik (0,84; p=0,02) e bok (1,77; p=0,0001) possuíam maior expressão no período pré-mob em relação aos indivíduos sadios (bid: 2,64; bik: 0,33; bok: 0,26). Não foram observadas diferenças significativas na expressão das moléculas da via extrínseca da apoptose nos pacientes com EM (p>0,05) nos períodos avaliados. Os valores de expressão de bcl-w, bak, bax, bik, bok e cIAP-1 atingiram níveis semelhantes aos controles após o transplante. A expressão dos genes bcl-2, cIAP-1, bad e bax estava maior nos pacientes em remissão da EM quando comparados àqueles em progressão neurológica. O aumento da expressão dos genes pró-apoptóticos bax, bak e bimEL correlacionou-se inversamente aos valores de EDSS dos pacientes com EM após o TACTH. Os resultados de expressão protéica foram equivalentes aos de expressão gênica nas duas doenças, com exceção dos dados das proteínas Bcl-2 e Bim. Em conjunto, os resultados demonstraram a desregulação da expressão de várias moléculas anti- e pró-apoptóticas nas CMN dos pacientes com DM-1 e EM. Esses achados sugerem a associação de alterações nos processos de apoptose celular com o surgimento e persistência de células auto-reativas no DM-1 e EM. Os dados indicam que essas alterações, principalmente a diminuição da expressão de moléculas pró-apoptóticas, como bak e bax, possam contribuir para a patogênese do DM-1 e EM. Além disso, a terapia de IAD/TACTH foi capaz de modular a expressão da maioria dos genes anormalmente expressos nas CMN dos pacientes com DM-1 e EM, já que esses atingiram níveis de expressão similares ao grupo controle após o transplante. Esta normalização da expressão de vários genes analisados correlacionou-se com a remissão clínica da doença na maioria dos pacientes / Type 1 diabetes mellitus (T1DM) and multiple sclerosis (MS) are inflammatory, organ-specific autoimmune diseases characterized by selective destruction of insulin-producing pancreatic -cells and central nervous system, respectively, by autoreactive B and T cells. Deregulation of apoptotic machinery is supposed to contribute to self-tolerance breakdown and autoimmune diseases pathogenesis, since apoptotic molecules have an important role in B and T lymphocytes central and peripheral tolerance mechanisms. The aim of this study was to evaluate the expression of pro and anti-apoptotic molecules from intrinsic and extrinsic apoptotic pathways and IAP Family members in 33 healthy individuals, 15 T1DM and 18 MS patients submitted to high-dose immunossupression therapy followed by autologous hematopoietic stem cell transplantation (HDI/AHSCT). Peripheral blood mononuclear cells (PBMC) were isolated from controls and patients at pre-mobilization (pre-mob), pre-conditioning (pre-cond), D+180, D+360, D+540 and D+720 post-transplantation. PBMC were used for RNA extraction, cDNA synthesis, gene quantification of a1, bcl-2, bcl-w, bcl-xL, bad, bak, bax, bid, bik, bimEL, bok, noxa, fas, fasL, c-FLIPL, cIAP-1 and cIAP-2 by Real Time PCR and Bcl-2, Bcl-xL, Bak, BimEL and c-FLIPL proteins detection by western-blotting. Results are expressed as median of relative expression units. Results from T1DM patients indicated that antiapoptotic molecules bcl-2 (median: 0,98; p=0,04), bcl-w (0,08; p=0,04), mcl-1 (1254; p=0,03) and cIAP-1 (1,24; p=0,003) were downregulated at pre-mob compared with healthy controls (medians bcl-2: 7,58; bcl-w: 0,52; mcl-1: 1659; cIAP-1: 14,5), while cIAP-2 (60,8; p=0,0005) gene expression was upregulated compared to healthy controls (23,3). We observed a significant decrease in proapoptotic bad (0,002; p<0,0001), bax (0,01; p=0,002) and fasL (1,66; p=0,001) genes expression in patients PBMC at pre-mob period compared to healthy subjects (bad: 0,23; bax: 2,79; fasL: 3,56). mRNA levels of bid (0.10; p=0.001) and bok (0.72; p=0.006) were elevated at pre-mob period when compared to control group (bid: 0.004; bok: 0.31). The bcl-2, bcl-w, bcl-xL, mcl-1, bad, bak, bax, bok, fasL and cIAP-1 mRNA levels reached controls levels after HDI/AHSCT. We observed that bcl-w, cIAP-1 and noxa gene expression were increased in T1DM patients in remission when compared to relapsed patients. The decreased antiapoptotic gene expression and increased in proapoptotic molecules correlated with decreased glicosilated hemoglobin percentages (Hb A1C) and anti-GAD65 antibodies and increased peptide-C levels. Results from MS patients showed decreased bcl-w (0,11; p=0,02) and cIAP-1 gene expression (1,87; p=0,04) in patients PBMC at pre-mob period compared to healthy controls (bcl-w: 0,27; cIAP-1: 7,75) and increased expression of a1 (90,8; p=0,001) and cIAP-2 (58,8; p=0,009) compared to controls (a1: 12,7; cIAP-2: 22,3). Proapoptotic molecules bad (0.007; p=0.01) and bax (0.0007; p=0.004) showed decreased gene expression at pre-mob compared to control group (bad: 0.27; bax: 1.24). bid (20.7; p=0.004), bik (0.84; p=0.01) and bok genes (1.77; p=0.0001) showed increased expression at pre-mob compared to healthy controls (bid: 2.64; bik: 0.33; bok: 0.26). Significant differences were not observed in the expression of the extrinsic pathway genes in pre-mob and healthy controls samples (p>0.05). bcl-w, bak, bax, bik, bok and cIAP-1 expression values reached healthy control values after transplantation. We observed that bcl-2, cIAP-1, bad and bax gene expression was increased in MS patients in disease remission when compared to patients with neurologic progression. Significant correlation of increased proapoptotic genes expression with decreased EDSS values in MS patients after HDI/AHSCT was observed. Results of protein quantification of apoptotic molecules in PBMC of T1DM and MS patients were similar to the gene expression results of these molecules, except for Bcl-2 and Bim proteins. Taken together, these data indicate a deregulated expression of anti- and proapoptotic genes in T1DM and MS patients PBMC. These data suggest an association of deregulated apoptosis with emergence and maintenance of autoreactive lymphocytes in analyzed patients. Based on these results, we suggest that this altered gene expression profile, mainly the decreased proapoptotic genes expression, as bak and bax, may contribute to T1DM and MS pathogenesis. Furthermore, we showed that the HDI/AHSCT therapy was able to modulate and normalize the expression of most genes abnormally expressed in T1DM and MS patients at pre-transplant period. Many analyzed genes achieved expression levels similar to healthy controls. The normalization of the expression of many evaluated genes correlated to disease remission in the majority of the patients.
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