Análise da expressão gênica por microarrays de células-tronco hematopoéticas e mesenquimais de pacientes com esclerose múltipla / Gene expression profiles of hematopoietic stem cells and mesenchymal stromal cells obtained from multiple sclerosis patients and detected by microarrays.

Oliveira, Gislane Lelis Vilela de

22 February 2013

As células-tronco hematopoéticas (CTHs) e estromais mesenquimais multipotentes (CTMs) isoladas da medula óssea vêm sendo utilizadas como fonte autóloga no tratamento de doenças autoimunes, como a esclerose múltipla (EM). As CTHs dão origem a todas as células dos sistemas hematopoético e imunológico e as CTMs possuem propriedades imunomoduladoras pela liberação de fatores solúveis e interação célula-célula. Existem trabalhos que sugerem que as doenças autoimunes sejam provenientes de defeitos intrínsecos nas células-tronco precursoras da medula óssea. Com o intuito de avaliar se as CTHs e CTMs de pacientes com EM possuem alterações intrínsecas, o objetivo geral deste trabalho foi avaliar o perfil de expressão gênica diferencial por microarrays de CTHs e CTMs de pacientes com EM, além de avaliar o perfil de expressão gênica de CTMs após o transplante autólogo de CTHs e a capacidade imunomoduladora in vitro das CTMs de pacientes. As CTHs e CTMs foram isoladas da medula óssea de pacientes com EM e doadores saudáveis, após consentimento informado. As CTHs foram isoladas por colunas imunomagnéticas e as CTMs foram isoladas por gradiente de densidade e submetidas à caracterização morfológica, imunofenotípica e capacidade de diferenciação em adipócitos e osteócitos. O RNA das CTHs e CTMs foi extraído e purificado e o perfil de expressão gênica foi avaliado por microarrays, utilizando hibridações em lâminas contendo 44.000 sondas. A capacidade imunomoduladora das CTMs de pacientes e controles foi avaliada por ensaios de cocultivo com linfócitos alogênicos e as citocinas foram quantificadas no sobrenadante por CBA flex e ELISA. Este estudo foi aprovado pelo comitê de ética do Hospital das Clínicas da Faculdade de Medicina de Ribeirão Preto. Os resultados mostraram que as CTHs de pacientes possuem perfis de expressão gênica diferentes dos controles, com 2.722 genes diferencialmente expressos, envolvidos em vias de sinalização importantes para manutenção/proliferação das CTHs e diferenciação em linhagens específicas durante a hematopoese. Dentre essas sinalizações estão incluídas as vias da apoptose, Wnt, Notch, mTOR, PI3K/Akt e Ca/NFAT, sugerindo que as CTHs de pacientes com EM possuam alterações intrínsecas que podem estar relacionadas com a patogenia da doença autoimune. As CTMs isoladas de pacientes com EM exibiram aparência senescente e reduzida expressão de marcadores imunofenotípicos. Com relação à expressão gênica, as CTMs de pacientes possuem perfil diferente das CTMs controle, sendo detectados 618 genes diferencialmente expressos, incluindo genes relacionados à sinalização FGF, HGF, sinalização de moléculas de adesão e moléculas envolvidas nos processos de imunorregulação, como IL10, IL6, TGFB1, IFNGR1, IFNGR2 e HGF. O perfil de expressão gênica das CTMs de pacientes pós-transplante assemelhou-se ao perfil das CTMs pré-transplante. Ensaios de cocultivo de CTMs com linfócitos alogênicos mostraram que as CTMs de pacientes possuem capacidade antiproliferativa reduzida em relação às CTMs controle, e ainda, secreção reduzida de TGF- e IL-10 no sobrenadante das coculturas. Esses dados sugerem que as CTMs isoladas de pacientes com EM possuam alterações fenotípicas, transcricionais e funcionais. Embasados nesses achados, concluímos que as CTHs e as CTMs de pacientes com EM possuem alterações intrínsecas que podem estar relacionadas com a patogenia da doença. Uma vez que as CTMs sejam células com grande potencial terapêutico para controle da EM em pacientes refratários aos tratamentos convencionais, as alterações encontradas sugerem que CTMs de doadores saudáveis sejam mais adequadas em aplicações clínicas. / Bone marrow hematopoietic stem cells (HSCs) and mesenchymal stromal cells (MSCs) have been used as an autologous source to treat autoimmune diseases, such as multiple sclerosis (MS). HSC give rise to all hematopoietic and immune system cells, and MSCs exhibit immunomodulatory properties by releasing soluble factors and by cell-cell interactions. Evidence indicates that bone marrow stem cells obtained from patients with autoimmune diseases may present intrinsic defects. To assess whether or not HSC and MSC of MS patients have intrinsic defects, the main objective of this study was to evaluate the differential gene expression profiles of HSC and MSC from MS patients before and after autologous HSC transplantation, and additionally, to evaluate the in vitro immunomodulatory ability of patient MSCs. Bone marrow HSC and MSCs were isolated from MS patients and healthy donors. HSCs were isolated by immunomagnetic columns and MSCs were isolated by gradient density and cultured until the third passage. MSCs were characterized according to morphology, immunophenotypic markers and cell differentiation into adipocytes and osteocytes. HSC and MSCs mRNAs were extracted, purified, and the gene expression profile was evaluated by microarray hybridizations, using a platform containing 44.000 probes. The immunomodulatory activity of patient and control MSCs was assessed by coculture assays with allogeneic lymphocytes. Cytokines were quantified in coculture supernatants by ELISA and CBA flex. This study was approved by the Ethics Committee of the University Hospital of the School of Medicine of Ribeirão Preto. The results showed that the patient HSCs exhibited a distinctive gene expression profile when compared to healthy HSCs, yielding 2.722 differentially expressed genes, involved in essential HSC signaling pathways for maintenance, proliferation and differentiation into specific lineages during hematopoiesis. Among these signaling pathways were included, apoptosis, Wnt, Notch, mTOR, PI3K/Akt and Ca/NFAT, suggesting that patient HSCs have significant intrinsic transcriptional alterations that may be associated with MS pathogenesis. Regarding MSCs isolated from MS patients, they exhibited senescence appearance, decreased expression of immunophenotypic markers, and also exhibited a distinctive gene expression profile in relation to healthy MSCs, yielding 618 genes differentially expressed genes, included in FGF and HGF signaling pathways, adhesion molecules, and genes involved in immunoregulation processes, such as IL-10, IL-6, TGFB1, IFNGR1, IFNGR2 and HGF. Coculture assays of control or patient MSCs with allogeneic lymphocytes showed that patient cells exhibited reduced antiproliferative activity as compared with controls, and also exhibited reduced secretion of TGF- and IL-10 cytokines in coculture supernatants. These data suggest that MSCs isolated from MS patients have phenotypic, functional and transcriptional defects, highlighting genes related to MSC maintenance, adhesion and immunomodulatory effects. According to these results, we concluded that patient HSCs and MSCs have intrinsic defects that may be associated with the disease per se. Considering that MSCs exhibit great therapeutic potential to control MS patients refractory to conventional treatment, the major MSCs alterations observed in this study indicate that healthy MSCs may be more suitable for MS cell therapy.

autoimmune diseases

células-tronco hematopoéticas

differential gene expression profile

doenças autoimunes

esclerose múltipla

expressão gênica diferencial

hematopoietic stem cells

multiple sclerosis

multipotent mesenchymal stromal cells

The implication of natural killer cells and neutrophils in autoimmune disorders of the central nervous system

Hertwig, Laura

05 September 2016

Die genaue Implikation natürlicher Killer(NK)-zellen und Neutrophile in Autoimmunerkrankungen des zentralen Nervensystems (ZNS) ist nach wie vor ungeklärt und wurde daher im Mausmodell der multiplen Sklerose (MS), der experimentellen Autoimmunenzephalomyelitis (EAE), sowie bei MS und Neuromyelitis optica (NMO) Patienten untersucht. Bei MS Patienten konnte eine mit der Krankheitsaktivität korrelierende, reduzierte Zahl zirkulierender CX3CR1+NK Zellen festgestellt werden. Daher wurden die NK Zell-Dynamiken und der Einfluss von CX3CR1 auf diese im EAE Mausmodell untersucht. Hierbei konnte in Wildtyp(WT) sowie auch CX3CR1-defizienten EAE Mäusen eine Rekrutierung peripherer NK Zellen in das ZNS beobachtet werden. Anders als bei WT EAE Mäusen wiesen die NK Zellen bei CX3CR1-defizienten Mäusen einen primär unreifen Phänotyp auf, der möglicherweise als ursächlich für die erhöhte Krankheitsaktivität dieser Tiere gemutmaßt werden kann. Der Transfer reifer NK Zellen vor Immunisierung CX3CR1-defizienter Tiere zeigte folglich protektive Effekte und lässt schlussfolgern, dass die CX3CR1-vermittelte Rekrutierung reifer NK Zellen die EAE Neuroinflammation limitiert. Die Diskriminierung der MS von der klinisch ähnlichen NMO stellt nach wie vor eine Herausforderung dar. Neutrophile in ZNS-Läsionen und der Cerebrospinalflüssigkeit(CSF) können bei NMO, nicht aber MS Patienten nachgewiesen werden, weshalb Neutrophile aus dem Blut von NMO und MS Patienten hier vergleichend untersucht wurden. Die Neutrophile beider Patientengruppen wiesen einen aktivierten Phänotyp im Vergleich zu gesunden Kontrollen auf. Im Gegensatz dazu zeigte sich eine von Medikation und neurologischen Defiziten der Patienten unabhängige, kompromittierte Funktionalität der NMO verglichen mit MS Neutrophilen im Hinblick auf Migration, oxidativen Burst und Degranulierung. Die Neutrophilenfunktionalität könnte entsprechend potentiell als diagnostisches Diskriminierungskriterium zwischen der MS und der NMO dienen. / The implication of natural killer (NK) cells and neutrophils in autoimmune disorders of the central nervous system (CNS) remains elusive, and therefore was investigated in a mouse model for multiple sclerosis (MS), experimental autoimmune encephalomyelitis (EAE), and in patients with MS and neuromyelitis optica (NMO), respectively. In MS, a decreased frequency of circulating CX3CR1+NK cells correlating with the patient disease activity has been reported. Therefore, the pattern of NK cell mobilization and the contribution of CX3CR1 to NK cell dynamics in response to neuroinflammatory insult were investigated in the EAE model. Here, NK cells similarly mobilized from the periphery and accumulated in the CNS in both wild-type (WT) and CX3CR1-deficient mice during EAE. However, in mice lacking CX3CR1 the infiltrated NK cells displayed an immature phenotype contrasting with the mature infiltrates in the WT counterparts, apparently contributing to EAE exacerbation in those animals since transfer of mature WT NK cells prior to immunization of CX3CR1-deficient mice exerted a protective effect. Together, these data suggest that the CX3CR1-mediated recruitment of mature CX3CR1+NK cells limits EAE neuroinflammation. Due to clinical similarities, the discrimination between MS and NMO is still challenging. In contrast to MS, neutrophil accumulations were found in CNS lesions and the cerebrospinal fluid (CSF) of NMO patients wherefore a comparative analysis of peripheral blood neutrophils in NMO and MS patients was performed. The results revealed an activated neutrophil phenotype in NMO and MS when compared to healthy individuals. In contrast, analysis of neutrophil migration, oxidative burst activity and degranulation showed a compromised neutrophil functionality in NMO compared to MS, which was not influenced by the treatment regime and clinical parameters of the patients. Thus, neutrophil functionality may represent a new diagnostic tool to discriminate between NMO and MS.

Natürliche Killerzellen

Neutrophile

ZNS Autoimmunerkrankungen

Multiple sklerose

Neuromyelitis optica

angeborene Immunzellen

multiple sclerosis

innate immunity

natural killer cells

CNS autoimmune diseases

neuromyelitis optica

neutrophils

570 Biowissenschaften, Biologie

32 Biologie

XG 4493

WW 4200

ddc:570

Prescribing patterns of biologic immunomodulating medicine in the South African private health care sector / Ilanca Roux

Roux, Ilanca

January 2010

Advances in molecular immunology and rapid technical evolution during the past two decades have led to a new class of medicines called biologics. Recently, a large number of biologics, or biologic immunomodulators, directed towards an array of immune–mediated diseases, have entered the market. This has lead to a dramatic change in the immunotherapy of autoimmune diseases, as biologics present new potential to improve or substitute conventional immunosuppressive therapies. According to literature, biologics are used by only a small number of a health plan’s members, (approximately one per cent), but a single occurrence can be relatively expensive. Furthermore, there is an indication that the frequency of use and cost of biologics are on the rise, and as more biologics enter the market, health plans and employers face the challenge of controlling costs while ensuring that biologics are affordable. The general objective of this study was to determine the prevalence and cost of biologic immunomodulating medicine in the treatment of certain autoimmune diseases during the period 2005 to 2008 in a section of the private health care sector of South Africa, by employing a medicine claims database as a source to obtain necessary information. A quantitative, retrospective drug utilisation review (rDUR) was performed on computerised medication records (medicine claims data) for four consecutive years (i.e. 2005 to 2008) provided by a pharmacy benefit management company (PBM). The study population consisted of all patients on the database who received at least one medicine item with adalimumab, etanercept, infliximab, interferon beta–1a, interferon 1–b or rituximab as active ingredient and who were diagnosed with either rheumatoid arthritis (RA), multiple sclerosis (MS) or Crohn’s disease between 1 January 2005 and 31 December 2008. Between 2005 and 2008, an average of 1,305,201 patients appeared on the total database, and of these 0.055% (n = 713) received biologic immunomodulating medicine. More than two thirds of biological users were female and most patients who received these medicine items were between the ages of 39 and 64 years, followed by those patients aged between 25 and 39 years. Biologic immunomodulating medicine items (n = 11,914) and biologic prescriptions (n = 9,537) represented 0.016% of the total number of medicine items (N = 76,129,173) and 0.030% of the total number of prescriptions (N = 31,985,153). The percentage contribution of biologic immunomodulators to the total number of medicine items and prescriptions on the total database increased each year, and in four years’ time the percentage of all the medicine items on the total database that included biologic immunomodulators had tripled, from 0.009% to 0.023%. The total cost of biologic immunomodulating medicine accounted for 1.278% of the total cost (N = R7, 483,759,176.23) of all medication claimed through the PBM between 2005 and 2008. The percentage contribution of biologic immunomodulators to the total medicine expenditure also increased from one year to another for the four–year study period. The average cost of a biologic immunomodulating medicine item increased with 71.10% from 2005 (R5602.71 ± 2166.61) to (R9586.25 ± 5956.56) in 2008. The CPI for biologic immunomodulators, (CPI = 60.00 for 2005; CPI = 74.62.17 for 2006; CPI = 85.26 for 2007; and CPI = 86.96 for 2008) indicated that biologic immunomodulating medicine items were relatively expensive and the d–value between the average cost per biologic immunomodulator and the average cost per non–biological medicine item (d–value = 2.54 in 2005, d–value = 3.32 in 2006, d–value = 2.23 in 2007 and d–value = 1.59 in 2008) furthermore indicated that the impact of biological therapies was large and practically significant. Rheumatoid arthritis patients represented 19.78% of the total number of patients (n = 713) who claimed the biologic immunomodulators during the four–year period, MS patients (n = 172) represented 24.12% and Crohn’s patients (n = 11) represented 1.5%. Biological drugs prescribed to RA patients represented 0.28% (n = R20, 708,818.82) of the total cost (N = R7, 483,759,176.23) of all medication claimed through the PBM during the four–year period, while those prescribed to MS patients represented 0.41% (R30, 922,520.07) and those prescribed to Crohn’s disease patients represented 0.015% (R1, 108,568.02). Although biologic immunomodulating medicine items used in the treatment of RA, MS and Crohn’s disease are relatively expensive, it seems that the number of other medication prescribed to patients with these diseases decreased after treatment with biologics, which may influence the medicine treatment cost of these patients. It can be concluded that even though biologic immunomodulators are used by only a very small percentage of the total patient population in a section of the private health care sector of South Africa, they are relatively expensive and have a considerable impact not only the medical aid scheme, but also on the patient. / Thesis (M.Pharm (Pharmacy Practice))--North-West University, Potchefstroom Campus, 2011.

Biologics

Biologic immunomodulating medicine

Biological medicine

Autoimmune diseases

Rheumatoid arthritis

Multiple sclerosis

Crohns disease

Pharmacoeconomics

Drug utilisation review

Biologiese produkte

Biologiese immunomodulerende medisyne

Biologiese medisyne

Outo-immuun siektes

Rumatoïde artritis

Veelvuldige sklerose

Crohn se siekte

Farmako-ekonomie

Medisyneverbruiksevaluering

Prescribing patterns of biologic immunomodulating medicine in the South African private health care sector / Ilanca Roux

Roux, Ilanca

January 2010

Advances in molecular immunology and rapid technical evolution during the past two decades have led to a new class of medicines called biologics. Recently, a large number of biologics, or biologic immunomodulators, directed towards an array of immune–mediated diseases, have entered the market. This has lead to a dramatic change in the immunotherapy of autoimmune diseases, as biologics present new potential to improve or substitute conventional immunosuppressive therapies. According to literature, biologics are used by only a small number of a health plan’s members, (approximately one per cent), but a single occurrence can be relatively expensive. Furthermore, there is an indication that the frequency of use and cost of biologics are on the rise, and as more biologics enter the market, health plans and employers face the challenge of controlling costs while ensuring that biologics are affordable. The general objective of this study was to determine the prevalence and cost of biologic immunomodulating medicine in the treatment of certain autoimmune diseases during the period 2005 to 2008 in a section of the private health care sector of South Africa, by employing a medicine claims database as a source to obtain necessary information. A quantitative, retrospective drug utilisation review (rDUR) was performed on computerised medication records (medicine claims data) for four consecutive years (i.e. 2005 to 2008) provided by a pharmacy benefit management company (PBM). The study population consisted of all patients on the database who received at least one medicine item with adalimumab, etanercept, infliximab, interferon beta–1a, interferon 1–b or rituximab as active ingredient and who were diagnosed with either rheumatoid arthritis (RA), multiple sclerosis (MS) or Crohn’s disease between 1 January 2005 and 31 December 2008. Between 2005 and 2008, an average of 1,305,201 patients appeared on the total database, and of these 0.055% (n = 713) received biologic immunomodulating medicine. More than two thirds of biological users were female and most patients who received these medicine items were between the ages of 39 and 64 years, followed by those patients aged between 25 and 39 years. Biologic immunomodulating medicine items (n = 11,914) and biologic prescriptions (n = 9,537) represented 0.016% of the total number of medicine items (N = 76,129,173) and 0.030% of the total number of prescriptions (N = 31,985,153). The percentage contribution of biologic immunomodulators to the total number of medicine items and prescriptions on the total database increased each year, and in four years’ time the percentage of all the medicine items on the total database that included biologic immunomodulators had tripled, from 0.009% to 0.023%. The total cost of biologic immunomodulating medicine accounted for 1.278% of the total cost (N = R7, 483,759,176.23) of all medication claimed through the PBM between 2005 and 2008. The percentage contribution of biologic immunomodulators to the total medicine expenditure also increased from one year to another for the four–year study period. The average cost of a biologic immunomodulating medicine item increased with 71.10% from 2005 (R5602.71 ± 2166.61) to (R9586.25 ± 5956.56) in 2008. The CPI for biologic immunomodulators, (CPI = 60.00 for 2005; CPI = 74.62.17 for 2006; CPI = 85.26 for 2007; and CPI = 86.96 for 2008) indicated that biologic immunomodulating medicine items were relatively expensive and the d–value between the average cost per biologic immunomodulator and the average cost per non–biological medicine item (d–value = 2.54 in 2005, d–value = 3.32 in 2006, d–value = 2.23 in 2007 and d–value = 1.59 in 2008) furthermore indicated that the impact of biological therapies was large and practically significant. Rheumatoid arthritis patients represented 19.78% of the total number of patients (n = 713) who claimed the biologic immunomodulators during the four–year period, MS patients (n = 172) represented 24.12% and Crohn’s patients (n = 11) represented 1.5%. Biological drugs prescribed to RA patients represented 0.28% (n = R20, 708,818.82) of the total cost (N = R7, 483,759,176.23) of all medication claimed through the PBM during the four–year period, while those prescribed to MS patients represented 0.41% (R30, 922,520.07) and those prescribed to Crohn’s disease patients represented 0.015% (R1, 108,568.02). Although biologic immunomodulating medicine items used in the treatment of RA, MS and Crohn’s disease are relatively expensive, it seems that the number of other medication prescribed to patients with these diseases decreased after treatment with biologics, which may influence the medicine treatment cost of these patients. It can be concluded that even though biologic immunomodulators are used by only a very small percentage of the total patient population in a section of the private health care sector of South Africa, they are relatively expensive and have a considerable impact not only the medical aid scheme, but also on the patient. / Thesis (M.Pharm (Pharmacy Practice))--North-West University, Potchefstroom Campus, 2011.

Biologics

Biologic immunomodulating medicine

Biological medicine

Autoimmune diseases

Rheumatoid arthritis

Multiple sclerosis

Crohns disease

Pharmacoeconomics

Drug utilisation review

Biologiese produkte

Biologiese immunomodulerende medisyne

Biologiese medisyne

Outo-immuun siektes

Rumatoïde artritis

Veelvuldige sklerose

Crohn se siekte

Farmako-ekonomie

Medisyneverbruiksevaluering

The genetic basis of veno-occlusive disease with immunodeficiency syndrome

Roscioli, Tony, Clinical School - Prince of Wales Hospital, Faculty of Medicine, UNSW

January 2007

This thesis addresses the genetic basis of a rare autosomal recessive primary immunodeficiency disorder with the characteristic additional feature of venoocclusive disease of the liver (VODI). The interest in this condition was stimulated both by the potential to identify the genetic basis of a rare immunodeficiency and the opportunity to gain an insight into the biological basis of hepatic veno-occlusive disease, a poorly understood condition that is encountered most frequently in Australia as a consequence of bone marrow transplantation. The gene responsible for VODI was identified by homozygosity mapping and DNA sequence analysis of positional candidates and was shown to be the PML Nuclear Body expressed protein Sp110. This is the first time a PML Nuclear Body protein has been shown to be involved in immunodeficiency disorder. Subsequent immunofluorescence studies of affected patient cell lines showed absence of Sp110 in patient B cells. The role of SP110 alleles in the susceptibility of bone marrow transplant patients to hepatic veno-occlusive disease was investigated using a cohort of patients from the Fred Hutchinson Cancer Center, Seattle. A SNP association study identified initial evidence for an association, but the study lacked sufficient power after correction for multiple testing. Contemporaneously, Dr Igor Kramnik published a report that the murine homologue of Sp110, Ifi75 (also termed Ipr1) was deleted in mice that were supersusceptible to infection with Mycobacterium tuberculosis. A further SNP association study was therefore performed utilising a NSW cohort of Mantouxpositive South East Asian migrants, which detected evidence that alleles of SP110 may be associated with progression of M. tuberculosis infection. Again, the limited size of this cohort precluded definitive findings.

Liver -- Diseases -- Genetic aspects.

Liver -- Immunology.

Autoimmune diseases -- Genetic aspects.

Caractérisation des lymphocytes B régulateurs chez l'Homme / Characterization of human regulatory B cells

Simon, Quentin

13 November 2015

Le potentiel régulateur des lymphocytes B (LB), largement associé avec la production d’interleukine-10 (IL-10), a été mis en évidence dans des modèles murins de pathologies spécifiques d’Ag. Les cellules B transitionnelles (Tr.) CD24fortes CD38fortes ont été décrites comme régulatrices, au travers de la production d’IL-10, de l’inhibition de la prolifération T, ainsi que de la suppression de la réponse inflammatoire des cellules T. Les LB transitionnels représentent un stade de développement central dans la maturation des cellules B, en faisant le lien entre les cellules immatures de la moelle osseuse et celles matures situées dans les organes lymphoïdes secondaires. Dans une première étude, nous montrons que cette population est hétérogène, et composée de LB Tr. de type 1 (T1), T2, T3 et Tr. CD27+. Les LB T3 anergiques semblent jouer un rôle dans la tolérance périphérique en limitant la prolifération des lymphocytes T (LT) CD4+, tandis que les LB Tr. CD27+ IL-10+ nouvellement décrits inhibent la différenciation des LT CD4+ en cellules productrices d’IFN-γ et de TNF-α. Notons que les LB T1 et Tr. CD27+ se différencient rapidement en cellules productrices d’Ac suite à la reconnaissance de signaux de l’immunité innée. La production d’IL-10 est en partie dépendante des signaux perçus, provenant du microenvironnement. Nous avons décrit dans un second travail que les LB s’adaptent aux cellules avec lesquelles ils sont cultivés. En effet, les cellules B régulent spécifiquement les LT CD4+ mémoires (et non naïfs), en limitant leur prolifération avant d’induire une mort cellulaire. Ces caractéristiques fonctionnelles pourraient être associées avec une modification du programme transcriptionnel, permise par la plasticité des cellules B, qui se polarisent en LB régulateurs (Breg) de façon ciblée. L’expression des gènes PRDM1 et IL10 serait associée avec une signature Breg spécifique en culture mixte autologue, en opposition avec celle des gènes NFκB1 et BCL6. La transplantation rénale est un excellent modèle physiopathologique, pour étudier l’importance de certaines populations de LB dans la tolérance immunologique. L’étude BHL (B lymphocytes in humoral rejection and alloimmunisation) nous a permis de confirmer que les LB Tr. ont probablement un rôle important dans cette tolérance du greffon. La présence d’anticorps spécifiques du donneur (DSA) semble limiter l’émergence des LB Tr., même si le pourcentage de cellules B CD24fortes CD38fortes n’est a priori pas associé avec la capacité du compartiment lymphocytaire B à réguler la prolifération des cellules T des patients alloimmunisés. / Regulatory B cells (Breg) were first reported to be interleukine-10 (IL-10) producing B cells in mice. The almost concurrent discovery of Breg cells drew interest toward potential links with transitional B cells because of phenotypic and functional similarities. In addition with IL-10 production, CD24high CD38high transitional B cells limit the proliferation of T cells and the polarization of CD4+ T cells into Th1 cells. Transitional B cells represent a central developmental stage in B-cell maturation, linking generation in the bone marrow with differentiation in periphery. In a first study, we reveal for the first time that human transitional B cells encompass not only transitional type 1 and type 2 B cells, but also distinct anergic type 3 B cells, as well as IL-10-producing CD27+ transitional B cells. Interestingly, the latter two subsets differentially regulate CD4+ T-cell proliferation and polarization toward Th1 effector cells. Additional experiments showed that type 1 and CD27+ transitional B cells are capable to differentiate into antibody secreting cells after toll-like receptor 9 engagement. In a second work, we wanted to explore the ability of B cells to target T-cell populations. We demonstrate that B cells can be suppressive cells. B cells are capable to target CD4+ memory T-cell, limiting the proliferation and inducing the death of this T-cell population. At the opposite, B cells seem to be effector of CD4+ naïve T-cell functions. These properties are probably associated with a specific transcriptional program. Thus, we observed that suppressive B cells overexpress PRDM1 and IL10, whereas effector B cells preferentially express BCL6 and NFκB1 in in vitro mixed culture. In the last part, we worked on B-cell phenotype and functions in transplanted patients. BHL (B lymphocytes in humoral rejection and alloimmunisation) is a clinical study that aims to better understand the role of B cells in the alloimmunisation and the chronic rejection occurring after renal transplantation. Donor specific antibodies (DSA) seem to limit the expansion of transitional B cells, which are probably not associated with the ability of B cells to regulate T-cell proliferation in DSA+ patients.

Lymphocytes B régulateurs

Cellules B transitionnelles

Interleukine 10

Anergie

Lymphocytes T

Maladies autoimmunes

Transplantation rénale

Alloimmunisation

Bioinformatique

Regulatory B cells

Transitional B cells

Interleukin 10

Anergy

T cells

Autoimmune diseases

Renal transplantation

Alloimmunisation

Bioinformatic softwares

571.967

Caracterização de autoanticorpos associados ao padrão de imunofluorescência “Rods & Rings” em pacientes infectados com o vírus da Hepatite C / Characterization of autoantibodies associated with the immunofluorescence pattern "Rods & Rings" in patients infected with Hepatitis C

Keppeke, Gerson Dierley [UNIFESP]

27 July 2011

Made available in DSpace on 2015-07-22T20:49:40Z (GMT). No. of bitstreams: 0 Previous issue date: 2011-07-27 / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / Introdução: Pacientes com Hepatite C frequentemente tendem a produzir autoanticorpos. No teste fator antinúcleo em células HEp-2 (ANA-HEp-20), esses autoanticorpos geram diversos padrões de imunofluorescência, sendo o nuclear pontilhado fino o mais frequente deles. Recentemente, tem sido descrito um novo padrão de ANA-HEp-2 em pacientes com HCV, denominado padrão Rods e Rings (R&R), caracterizado por anéis e bastões. Objetivos: Avaliar as características clínicas, virológicas e padrão de resposta terapêutica dos pacientes que apresentam autoanticorpos que geram o padrão R&R, bem como proceder a uma avaliação preliminar dos aspectos celulares e moleculares desse novo sistema de autoantígenos. Métodos: Amostras de soro coletadas de 1998 até 2008 de 597 pacientes foram submetidas ao teste de ANA-HEp-2 em lâminas Euroimmun ou INOVA e classificados como R&R positivos quando apresentaram fluorescência sob forma de bastões de 3 a 10μm de comprimento e anéis de 2 a 5μm de diâmetro no citoplasma das células HEp-2. Entre os pacientes testados, 342 tinham HCV e 200 tinham outras doenças hepáticas crônicas ou autoimunes reumáticas, além de 55 pacientes co-infectados com HCV+HIV. As informações clínicas, virológicas e terapêuticas foram coletadas de bancos de dados atrelados às amostras de soro dos pacientes. Células HEp-2, 3T3 e MH22A foram cultivadas normalmente e/ou submetidas à tratamentos in vitro (tripsina e ribavirina) e com dois métodos alternativos de fixação, para estudo das estruturas do R&R por imunofluorescência indireta simples ou com técnicas de dupla-marcação com amostras R&R-positivas e anticorpos antitubulina-alfa e anti-CTP-sintase. Resultados: Dos 342 pacientes com HCV, 51 (15%) apresentaram o padrão R&R, enquanto que dos 200 pacientes com outras doenças hepáticas ou autoimunes, apenas um apresentou o padrão R&R (p<0.0001). Dos pacientes com HCV, 174 eram tratados e 168 não tratados. Dos 174 tratados, 49 (28%) apresentaram o padrão R&R contra apenas dois (1%) dos não tratados (p<0.0001). De 134 tratados e com informação adequada sobre a medicação utilizada, 108 tomavam interferon-α e ribavirina e 23 tomavam apenas interferon-α. Quarenta e um (38%) dos 103 que tomavam interferon-α e ribavirina apresentaram o padrão R&R contra nenhum (0%) dos 23 que tomavam apenas interferon-α (p= 0.0001). Quanto aos outros padrões de ANA-HEp-2, dos 23 pacientes que tomavam apenas interferon-α, 12 (52%) foram positivos enquanto apenas 27 (25%) dos que tomavam interferon-α e ribavirina foram positivos (p= 0.010). 9% dos pacientes co-infectados com HCV+HIV apresentaram o padrão R&R. Não encontramos relação entre a presença do padrão R&R e o genótipo do vírus, a carga viral e os dados demográficos dos pacientes com HCV. A porcentagem de respondedores ao tratamento foi ligeiramente menor nos pacientes que apresentaram o R&R, porem sem atingir nível de significância estatística (p=0,150). Lâminas ANA-HEp-2 de algumas marcas comerciais que não Euroimmun e INOVA e aquelas elaboradas no próprio laboratório não apresentaram as estruturas do R&R. Quando tratadas in vitro com ribavirina ou tripsina, as células HEp-2 ou 3T3 e MH22A de camundongo cultivadas expressaram vários anéis e bastões reconhecidos pelas amostras de soro R&R-positivas. Não observamos colocalização das estruturas R&R com microtúbulos e observamos fraca colocalização dos anéis e bastões com CTP-sintase. Conclusões: Autoanticorpos associados ao padrão R&R ocorreram em íntima associação ao uso de interferon-α e ribavirina em pacientes com hepatite HCV, independentemente de serem portadores do HIV. Não houve associação às características demográficas dos pacientes, ao perfil de resposta terapêutica, ao genótipo do HCV ou à carga viral. As estruturas em anéis e bastões associadas ao padrão R&R não ocorrem nas condições normais avaliadas, podendo ser induzidas in vitro pela exposição à ribavirina ou à tripsina. Há algum grau de conservação filogenética dos autoantígenos associados ao padrão R&R. Evidências preliminares indicam a presença da enzima CTP-sintase nas estruturas em anéis e bastões reconhecidas pelos autoanticorpos humanos. / Introduction: Patients with Hepatitis C frequently produce autoantibodies. In the antinuclear antibody assay on HEp-2 cells (ANA-HEp-2) these autoantibodies generate several immunofluorescence patterns, and the nuclear fine speckled pattern is the most common. A novel ANA-HEp-2 pattern has been recently reported, characterized by the presence of rods and rings in the cytoplasm. Objectives: To study the clinical and virological features, as well as the profile of therapeutic response of patients presenting autoantibodies generating the rods and rings (R&R) ANA-HEp-2 pattern and to perform a preliminary analysis of the cellular and molecular aspects of this novel autoantigen system. Methods: Serum samples obtained from 1988 to 2008 from 597 patients were processed in the ANA-HEp-2 assay on Euroimmun or INOVA slides and classified as R&R-positive when presenting immunofluorescence as 3-10μm long rods and 2-5μm diameter rings in the cytoplasm of HEp-2 cells. Among the tested patients, 342 had HCV, 200 had other chronic liver diseases or rheumatic autoimmune diseases, and 55 had HCV and HIV. Clinical, virological, and treatment information was obtained from the clinical data bank. Human HEp-2, and murine 3T3, and MH22A cell lines were cultured as usual and under special stimuli (exposure to trypsin or ribavirin), and prepared with alternative fixation protocols for processing in single or double indirect immunofluorescence with human anti-R&R serum and antibodies to tubulin and to CTP-synthase. Results: Among the 342 HCV patients, 51 (15%) presented the R&R pattern as opposed to only one among the 200 patients with other liver diseases and autoimmune rheumatic diseases (p<0.001). Among the HCV patients, 174 had been treated and 168 had received no treatment. Among the 174 treated patients, 49 (28%) presented the R&R pattern as opposed to only two (1%) of the 168 non-treated HCV patients (p<0.001). Among 134 HCV treated patients with detailed information on the treatment protocol, 108 used interferon-α and ribavirin and 23 used only interferon-α. Forty-one (38%) of the R&R pattern as opposed to none of the 23 patients receiving only interferon-α (p=0.0001). In contrast, 12 (52%) of the 23 patients receiving only interferon-α presented other non-R&R ANA-HEp-2 patterns as opposed to only 27 (25%) of the 108 patients under interferon-α and ribavirin (p=0.01). 9% of the patients with HCV and HIV presented the R&R pattern. There was no association between the occurrence of the R&R pattern and HCV genotype, viral load, and demographic features. The frequency of sustained virologic response was slightly lower in the R&R-positive patients but the difference did not reach statistical significance (p=0.15). ANA-HEp-2 slides from brands other than Euroimmun and INOVA, as well as in-house produced slides did not express the R&R structures. When treated in vitro with ribavirin or trypsin, HEp-2 cells and murine 3T3, and MH22A cell lines expressed prominent R&R structures recognized by human HCV serum samples. There was partial weak colocalization of CTP-synthase in the R&R structures but no colocalizadion of microtubule. Conclusions: autoantibodies associated with the R&R pattern were strongly associated with the use of interferon-α and ribavirin in patients with HCV, independently of co-infection with HIV. There was no association with demographic characteristics, the profile of therapeutic response, HCV genotype, and viral load. The rods and rings structures associated with the R&R pattern did not occur under normal conditions, but could be induced in vitro by exposure to ribavirin or trypsin. There is some degree of phylogenetic conservation of the autoantigens associated to the R&R pattern. Preliminary evidence indicates the presence of CTP-synthase in the cytoplasmic rods and rings structures recognized by human autoantibodies from HCV patients. / FAPESP: 2009/03796-5 / FAPESP: 2010/50710-6 / TEDE / BV UNIFESP: Teses e dissertações

Estruturas Citoplasmáticas

Hepatite C

Interferon alfa

Ribavirina

Autoanticorpos

Hepacivirus

Hepatopatias

Doenças Reumáticas

Doenças Autoimunes

Humanos

HIV

Cytoplasmic Structures

Hepatitis C

Interferon-alpha

Ribavirin

Autoantibodies

Hepacivirus

Liver Diseases

HIV

Rheumatic Diseases

Autoimmune Diseases

Humans

Estudo da região promotora do gene da interleucina (IL-21) e do poliformismo do gene tirosina fosfatase, tipo não receptor 22 (PTPN22): associação com auto-anticorpos em pacientes portadores de diabetes mellitos tipo 1A / Allelic variant in IL21 promoter region, C1858T PTPN22 frequency and autoantibodies in Brazilian type 1A diabetes patients

Debora Teixeira de Oliveira Mainardi Novo

11 August 2011

As citocinas têm papel importante como mediadores através das respostas imunológicas. A Interleucina-21, importante regulador dos linfócitos T e B, é produzida por linfócitos CD4 ativados, e está implicada na patogênese do diabetes autoimune em modelo animal, o NOD. A região promotora da IL-21, que contempla sítios de controle da expressão gênica em camundongos, o NFATc2, T-bet e c-MAF, foi estudada pela primeira vez em humanos portadores de diabetes tipo 1A, neste trabalho. Foi analisado também a freqüência do polimorfismo C1858T do gene PTPN22, que tem sido associado em estudos recentes como fator de risco importante para diabetes tipo1A e outras doenças autoimunes. Associou-se ainda, autoanticorpos pancreáticos e não-pancreáticos em diabéticos e grupo controle normal, e estes resultados foram analisados com ambos os genes. Foram estudados 612 DM1A e 792 indivíduos do grupo controle. Após extração de DNA genômico, a região 5proximal da região promotora do gene da Il-21, -448+83pb, foi seqüenciada em 309 brasileiros diabéticos tipo 1A e 189 indivíduos do grupo controle. A genotipagem do polimorfismo C1858T do gene PTPN22, por RFLP, foi realizada em 434 diabéticos e 689 controles, bem como os alelos HLA-DRB1. Foi encontrada uma variação alélica, em heterozigoze, na posição g.-241 T>A, em apenas uma paciente, que apresentou idade de diagnóstico aos 30 anos de idade. Esta variante alélica não foi encontrada nos 497 indivíduos (308 DM1A e 189 grupo controle). A freqüência dos alelos polimórficos (CT/TT) foi maior nos diabéticos (18.7%) que no grupo controle (10.6%), OR 1,94 e p<0,001. O polimorfismo C1858T do gene PTPN22 associou-se à maior freqüência dos autoanticorpos pancreático anti-GAD65 (p=0,002) e não-pancreático anti-TG (p=0,001), quando avaliados os dois grupos juntos, DM1A e grupo controle. Os diabéticos apresentaram maior freüência dos autoanticorpos como segue: autoanticorpos pancreáticos: anti-GAD65: 225 /482 (46.7%) vs 13/786 (1.7%), p<0.001; anti-IA2 : 204/469 (43.5%) vs 15/786 (1.9%), p<0.001. Autoanticorpos não-pancreáticos: FAN: 60/234 (25.6%) vs 13/239 (5.4%), p<0.001; anti-TPO: 64/279 (22.9%) vs 34/495 (6.9%), p<0.001; anti-TG : 65/278 (23.4%) vs 44/489 (9%), p<0.001; TRAb: 14/187 (7.5%) vs 1/327 (0.3%), p<0.001; anti-21-OH : 8/154 (5,2%) vs 1/160 (0,6%), p< 0,001. Os autoanticorpos a seguir foram realizados apenas nos pacientes diabéticos: anti-tTG 5/73% (6.8%), anti-Endom 10/176 (5.7%). Com exceção do anti-GAD65 e anti-TG, nenhum outro autoanticorpo associou-se ao polimorfismo do gene PTPN22. Os alelos HLA-DR3/DR$ predominaram nos diabéticos (p<0,001). Concluimos então que o polimorfismo C1858T do gene PTPN22 e os alelos HLA-DR3/DR4 estão associados ao risco de DM1A. Variantes alélicas na região 5 proximal do gene da IL-21 parece não ser predisponente à suscetibilidade ao DM1A e outras doenças autoimunes. Autoanticorpos órgão-específicos são mais freqüentes em diabéticos, principalmente nas glândulas adrenal e tireóide. O polimorfismo C1858T do gene PTPN22 está associado à maior freqüência dos autoanticorpos anti-GAD65 e antitireoglobulina / Objective: Cytokines are central mediators of inflammation through innate and adaptive immune responses. IL-21, a critical regulator of T and B cell function, is produced by various subsets of CD4+ T cells, and it has been implicated in the pathogenesis of non obese diabetes mouse. The proximal promoter of IL-21, which controls its Th-cell-subset-specific expression through the action of NFATc2, T-bet and c-MAF in animal models, was evaluated in type 1A diabetes (T1AD) patients for the first time. This study also analyzed the 1858T PTPN22 polymorphism, which has recently emerged as an important risk factor for T1AD and other autoimmune diseases. Moreover, islet and other organ-specific autoantibodies were quantified in T1AD patients and healthy controls and the results were correlated with both genes. Research design and methods: The case series comprised 612 T1AD patients and 792 healthy control (HC) individuals. Genomic DNA extraction was performed by salting-out in purified blood leukocytes. The region encompassing -448+83 bp of IL-21 gene was amplified and sequenced using genomic DNA from 309 Brazilian T1AD patients and 189 control individuals. RFLP genotyping of C1858T PTPN22 was performed in 689 controls and 434 T1D patients. HLA DR3/DR4 alleles were also evaluated. Results: A heterozygous allelic variant (g.-241 T>A) was found in only one patient, who was 30 years old at the onset of disease. This allelic variant was not found in 497 individuals (308 T1AD patients and 189 healthy controls). The PTPN22 1858T allele frequency was greater in patients (18.7%) than in controls (10.6%): odds ratio of 1.94; p<0.001. An association was found between C1858T polymorphism and higher frequency of GAD65 Ab (p=0.002) and TG Ab (p=0.011), among both T1AD and HC. Type 1 diabetes patients presented higher frequency of the following autoantibodies, compared with HC (p<0.001): GAD65 Ab (46.7% vs 1.7%); IA2 Ab (43.5% vs 1.9%); ANA (25.6% vs 5.4%); TPO Ab (22.9% vs 6.9%); TG Ab (23.4% vs 9.0%); TRAb (7.5% vs 0.3%); 21-OH Ab (5,2% vs 0,6%). The following antibodies were evaluated only in T1AD: tTG Ab (6.8%) anti-Endom (5.7%). Except by GAD65 Ab and TG Ab, no association was found between C1858T polymorphism and these autoantibodies.HLA-DR3/DR4 alleles predominated in T1D patients (p<0.001) Conclusions: C1858T PTPN22 polymorphism and the HLA-DR3 and/or DR4 alleles were associated with proneness to T1AD. Allelic variants at the 5\' proximal region of the IL-21 gene do not seem to predispose to susceptibility to T1AD and other autoimmune endocrine diseases. Autoantibodies specific to other organs and tissues are frequent in T1AD carriers, mainly to the thyroid glands. The 1858T PTPN22 polymorphism was associated with higher frequency of GAD65A and TGA.

Auto-anticorpos

Auto-imunidade

Citocinas

Diabetes mellitus tipo 1

Doenças auto-imunes

Interleucina-21

Polimorfismo genético

Autoantibodies

Autoimmune diseases

Autoimmunity

Cytokines

Diabetes mellitus type 1

Interleukin-21

Polymorphism genetic

Análise da expressão gênica por microarrays de células-tronco hematopoéticas e mesenquimais de pacientes com esclerose múltipla / Gene expression profiles of hematopoietic stem cells and mesenchymal stromal cells obtained from multiple sclerosis patients and detected by microarrays.

Gislane Lelis Vilela de Oliveira

22 February 2013

As células-tronco hematopoéticas (CTHs) e estromais mesenquimais multipotentes (CTMs) isoladas da medula óssea vêm sendo utilizadas como fonte autóloga no tratamento de doenças autoimunes, como a esclerose múltipla (EM). As CTHs dão origem a todas as células dos sistemas hematopoético e imunológico e as CTMs possuem propriedades imunomoduladoras pela liberação de fatores solúveis e interação célula-célula. Existem trabalhos que sugerem que as doenças autoimunes sejam provenientes de defeitos intrínsecos nas células-tronco precursoras da medula óssea. Com o intuito de avaliar se as CTHs e CTMs de pacientes com EM possuem alterações intrínsecas, o objetivo geral deste trabalho foi avaliar o perfil de expressão gênica diferencial por microarrays de CTHs e CTMs de pacientes com EM, além de avaliar o perfil de expressão gênica de CTMs após o transplante autólogo de CTHs e a capacidade imunomoduladora in vitro das CTMs de pacientes. As CTHs e CTMs foram isoladas da medula óssea de pacientes com EM e doadores saudáveis, após consentimento informado. As CTHs foram isoladas por colunas imunomagnéticas e as CTMs foram isoladas por gradiente de densidade e submetidas à caracterização morfológica, imunofenotípica e capacidade de diferenciação em adipócitos e osteócitos. O RNA das CTHs e CTMs foi extraído e purificado e o perfil de expressão gênica foi avaliado por microarrays, utilizando hibridações em lâminas contendo 44.000 sondas. A capacidade imunomoduladora das CTMs de pacientes e controles foi avaliada por ensaios de cocultivo com linfócitos alogênicos e as citocinas foram quantificadas no sobrenadante por CBA flex e ELISA. Este estudo foi aprovado pelo comitê de ética do Hospital das Clínicas da Faculdade de Medicina de Ribeirão Preto. Os resultados mostraram que as CTHs de pacientes possuem perfis de expressão gênica diferentes dos controles, com 2.722 genes diferencialmente expressos, envolvidos em vias de sinalização importantes para manutenção/proliferação das CTHs e diferenciação em linhagens específicas durante a hematopoese. Dentre essas sinalizações estão incluídas as vias da apoptose, Wnt, Notch, mTOR, PI3K/Akt e Ca/NFAT, sugerindo que as CTHs de pacientes com EM possuam alterações intrínsecas que podem estar relacionadas com a patogenia da doença autoimune. As CTMs isoladas de pacientes com EM exibiram aparência senescente e reduzida expressão de marcadores imunofenotípicos. Com relação à expressão gênica, as CTMs de pacientes possuem perfil diferente das CTMs controle, sendo detectados 618 genes diferencialmente expressos, incluindo genes relacionados à sinalização FGF, HGF, sinalização de moléculas de adesão e moléculas envolvidas nos processos de imunorregulação, como IL10, IL6, TGFB1, IFNGR1, IFNGR2 e HGF. O perfil de expressão gênica das CTMs de pacientes pós-transplante assemelhou-se ao perfil das CTMs pré-transplante. Ensaios de cocultivo de CTMs com linfócitos alogênicos mostraram que as CTMs de pacientes possuem capacidade antiproliferativa reduzida em relação às CTMs controle, e ainda, secreção reduzida de TGF- e IL-10 no sobrenadante das coculturas. Esses dados sugerem que as CTMs isoladas de pacientes com EM possuam alterações fenotípicas, transcricionais e funcionais. Embasados nesses achados, concluímos que as CTHs e as CTMs de pacientes com EM possuem alterações intrínsecas que podem estar relacionadas com a patogenia da doença. Uma vez que as CTMs sejam células com grande potencial terapêutico para controle da EM em pacientes refratários aos tratamentos convencionais, as alterações encontradas sugerem que CTMs de doadores saudáveis sejam mais adequadas em aplicações clínicas. / Bone marrow hematopoietic stem cells (HSCs) and mesenchymal stromal cells (MSCs) have been used as an autologous source to treat autoimmune diseases, such as multiple sclerosis (MS). HSC give rise to all hematopoietic and immune system cells, and MSCs exhibit immunomodulatory properties by releasing soluble factors and by cell-cell interactions. Evidence indicates that bone marrow stem cells obtained from patients with autoimmune diseases may present intrinsic defects. To assess whether or not HSC and MSC of MS patients have intrinsic defects, the main objective of this study was to evaluate the differential gene expression profiles of HSC and MSC from MS patients before and after autologous HSC transplantation, and additionally, to evaluate the in vitro immunomodulatory ability of patient MSCs. Bone marrow HSC and MSCs were isolated from MS patients and healthy donors. HSCs were isolated by immunomagnetic columns and MSCs were isolated by gradient density and cultured until the third passage. MSCs were characterized according to morphology, immunophenotypic markers and cell differentiation into adipocytes and osteocytes. HSC and MSCs mRNAs were extracted, purified, and the gene expression profile was evaluated by microarray hybridizations, using a platform containing 44.000 probes. The immunomodulatory activity of patient and control MSCs was assessed by coculture assays with allogeneic lymphocytes. Cytokines were quantified in coculture supernatants by ELISA and CBA flex. This study was approved by the Ethics Committee of the University Hospital of the School of Medicine of Ribeirão Preto. The results showed that the patient HSCs exhibited a distinctive gene expression profile when compared to healthy HSCs, yielding 2.722 differentially expressed genes, involved in essential HSC signaling pathways for maintenance, proliferation and differentiation into specific lineages during hematopoiesis. Among these signaling pathways were included, apoptosis, Wnt, Notch, mTOR, PI3K/Akt and Ca/NFAT, suggesting that patient HSCs have significant intrinsic transcriptional alterations that may be associated with MS pathogenesis. Regarding MSCs isolated from MS patients, they exhibited senescence appearance, decreased expression of immunophenotypic markers, and also exhibited a distinctive gene expression profile in relation to healthy MSCs, yielding 618 genes differentially expressed genes, included in FGF and HGF signaling pathways, adhesion molecules, and genes involved in immunoregulation processes, such as IL-10, IL-6, TGFB1, IFNGR1, IFNGR2 and HGF. Coculture assays of control or patient MSCs with allogeneic lymphocytes showed that patient cells exhibited reduced antiproliferative activity as compared with controls, and also exhibited reduced secretion of TGF- and IL-10 cytokines in coculture supernatants. These data suggest that MSCs isolated from MS patients have phenotypic, functional and transcriptional defects, highlighting genes related to MSC maintenance, adhesion and immunomodulatory effects. According to these results, we concluded that patient HSCs and MSCs have intrinsic defects that may be associated with the disease per se. Considering that MSCs exhibit great therapeutic potential to control MS patients refractory to conventional treatment, the major MSCs alterations observed in this study indicate that healthy MSCs may be more suitable for MS cell therapy.

células-tronco hematopoéticas

doenças autoimunes

esclerose múltipla

expressão gênica diferencial

autoimmune diseases

differential gene expression profile

hematopoietic stem cells

multiple sclerosis

multipotent mesenchymal stromal cells

Transcription factors and downstream genes modulating TNF-gas + IFN-gcs induced beta cell apoptosis

Barthson, Jenny

08 April 2013

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