Dissertations / Theses on the topic 'Transplantation immunology; Cellular rejection'

This thesis aims to place corneal allograft rejection in the context of general transplantation immunology, examine the role of lymphocyte subsets in the rejection process and consider the potential application of monoclonal antibody therapy in clinical corneal graft rejection. The literature relating to the current clinical practice of corneal grafting, with particular reference to corneal allograft rejection, is reviewed in chapter 1 to present the extent of the problem. Chapter 2 then reviews the mechanisms of allograft rejection from the literature of transplantation immunology, much of which has arisen from studies of kidney, heart, pancreatic islets and liver in animal models. The materials and methods are described in detail in chapter 3, and only the relevant experimental design is detailed in the Materials and Methods sections of the succeeding chapters. The experimental mouse model of transplanting corneal tissue into the renal subcapsular is evaluated in chapter 4, demonstrating that isografts survive indefinitely whereas allografts are rejected typically by 30 days. Pretransplant sensitisation decreased allograft survival time to 10 days. Immunohistochemistry demonstrated the presence of CD4⁺ and CD8⁺ lymphocytes and macrophages at the rejection site. Heterotopic corneal graft recipients were then treated with various monoclonal antibody regimes. Chapter 5 demonstrates that allograft survival can be increased by either anti-CD4 or anti-CD8 therapy, providing near total depletion of the respective lymphocyte subset is achieved. Xenograft rejection is shown to depend on mainly CD4⁺ lymphocytes in chapter 6, with no benefit being found of depleting the CD8⁺ subset in addition. A mild immunosuppressive effect of anti-Vβ8 monoclonal antibody is demonstrated and discussed in chapter 7. The final chapter discusses these results in the light of recent, related work in other transplant systems, and presents a case for a trial of intracameral pan-T-cell monoclonal antibody treatment.

The aim of this thesis was to investigate the effect of various parameters in patients with chronic liver disease pretransplant which may influence the occurrence of acute rejection post transplant. This may be useful in tailoring immunosuppression to avoid adverse effects in patients less likely to develop acute rejection. The role of cytokines in acute rejection is not clear but animal and human studies had suggested that tumour necrosis factor alpha (TNF-a) played some role. Polymorphisms in the genes encoding TNFa, interleukin 10 and transforming growth factor beta1 (TGFb1) which influence in vitro production of cytokines were examined in transplant patients. This showed an increase in the TNFa 2 polymorphism at position -308 in patients with acute rejection but no association with IL-10 or TGFb1 polymorphisms. Pretransplant levels of TNFa and IL-10 were measured following stimulation of peripheral blood mononuclear cells with lipopolysaccharide from patients with chronic liver disease. PBMC were preincubated with different immunosupressants. There was increased production of stimulated TNFa pretransplant in patients who went on to develop acute rejection. No relationship was found between IL-10 production and acute rejection. There were differences in the effects of tacrolimus, cyclosporin and dexamethasone on the production of both cytokines. The pretransplant immune status of patients was assessed by contact sensitisation to diphenylcyclopropenone (DPC). This demonstrated that patients unable to mount an immune response to DPC did not require treatment for acute rejection following liver transplantation. It also demonstrated a correlation between the strength of reaction to DPC and the severity of acute rejection.

Thesis (Ph.D. in Immunology) -- University of Colorado at Denver and Health Sciences Center, 2006.
Typescript. Includes bibliographical references (leaves 151-168). Free to UCDHSC affiliates. Online version available via ProQuest Digital Dissertations;

Lung transplantation is the only therapeutic approach for patients presenting end-stage pulmonary failure. Despite progress made in organ preservation and immunosuppression, primary graft dysfunction and obliterative bronchiolitis still hamper short-term and long-term outcomes, respectively. Interleukin-17 recently emerged as a major actor in several immuno-inflammatory disorders. Clinical and experimental evidence also suggest the implication of interleukin-17 or type 17 CD4+ T cells in lung rejection. We therefore investigated the contribution of this cytokine to graft pathology in a murine model of tracheal transplantation that recapitulates pathological features of lung rejection including the development of obliterative airway disease.

We first demonstrated that interleukin-17 contributes to inflammatory lesions in the early phase post-transplantation. Interleukin-17 was found to be produced by &61543;&61540;+ T cells and CD4+ T cells infiltrating the graft and interleukin-17 neutralization significantly reduced the development of epithelial lesions together with inhibition of interleukin-6 and heat-shock-protein 70 gene transcription.

We then investigated the contribution of interleukin-17 to obliterative airway disease. Although interleukin-17 did not play a dominant role in absence of immunosuppression, it was found to contribute to airway pathology in animals receiving cyclosporin A. Under this treatment, we first observed dramatic changes in the composition of the lymphocyte populations infiltrating the graft: the numbers of CD8+ T cells producing interferon-&61543; and type 1 CD4+ T cells were dramatically decreased while the numbers of type 17, and also type 2 CD4+ T cells were unaffected. The pathological relevance of these findings was first demonstrated by the prolongation of graft survival afforded by the depletion of CD4+ T cells in cyclosporin A-treated animals. Furthermore, graft rejection was also delayed in mice genetically deficient in either interleukin-17 or interleukin-4, providing evidence that type 17 and type 2 CD4+ T cells actively contribute to graft rejection in cyclosporin A-treated recipients. On the other hand, parallel experiments in interferon-&61543;-deficient mice revealed that interferon-&
Doctorat en Sciences médicales
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Lung transplantation is a therapeutic option for patients affected with end-stage lung diseases. However, several complications may arise following the procedure, such as Bronchiolitis Obliterans (BO). This condition, characterized by small airway fibrosis, remains a major cause of morbidity and mortality in patients following lung transplantation. It is thought to be a manifestation of chronic rejection within the airways, with hallmark inflammation and fibroproliferation. TGF-beta and other cytokines, including IL-1, IFN-gamma and PDGF, have been implicated in the pathogenesis of fibrosis, mostly in animal models. IL-11 and IL-17 are novel profibrotic cytokines that induce fibroblasts and epithelial cells to produce excess extracellular matrix. They have recently been identified as having a role in tissue remodelling and induction of tissue fibrosis. We hypothesize that IL-11 and IL-17 are involved in chronic lung rejection (Bronchiolitis Obliterans) and that their expression could be a predictive and prognostic marker of chronic lung rejection.
The objectives of the study were to investigate the expression of IL-11 and IL-17 (mRNA and protein) in endobronchial biopsies from lung transplant patients and to define the correlation between the expression of IL-11 and IL-17 and the development of chronic rejection.

Tolerance-based stem cell transplantation using sub-lethal conditioning is being considered for the treatment of human disease, but safety and efficacy remain to be established. In order to study these two issues, we first established that mouse bone marrow recipients treated with sub-lethal irradiation plus transient blockade of the CD40-CD154 costimulatory pathway develop permanent hematopoietic chimerism across allogeneic barriers. Our conditioning regimen of 6 Gy irradiation, a short course of anti-CD154 mAb and 25 million fully allogeneic BALB/c bone marrow cells consistently produced long-term, stable, and multilineage chimerism in C57BL/6 recipients. Furthermore, chimeric mice displayed donor-specific transplantation tolerance, as BALB/c skin allografts were permanently accepted while third-party CBA/JCr skin allografts were promptly rejected. We next determined both the safety and efficacy of this protocol by infecting chimeric mice with lymphocytic choriomeningitis virus (LCMV) either at the time of transplantation or at several time points afterwards. Infection with LCMV at the time of transplantation prevented engraftment of allogeneic, but not syngeneic, bone marrow in similarly treated mice. Surprisingly, infected allograft recipients also failed to clear the virus and died. Post-mortem study revealed hypoplastic bone marrow and spleens. Hypoplasia and death in these mice required the combination of 6 Gy irradiation, LCMV infection on the day of transplantation, and an allogeneic bone marrow transplant but did not require the presence of anti-CDl54 mAb. Allochimeric mice infected with LCMV 15 days after transplantation were able to survive and maintain their bone marrow graft, indicating that the deleterious effects of LCMV infection on host and graft survival are confined to a narrow window of time during the tolerization and transplantation process. The final section of this thesis studied the mechanisms of graft rejection and death in sublethally irradiated recipients of allogeneic bone marrow and infection with LCMV at the time of bone marrow transplantation. Infection of interferon-α/β receptor knockout mice at the time of transplantation prevented the engraftment of allogeneic bone marrow, but the mice survived. Therefore, IFN-αβ is involved in the development of marrow hypoplasia and death, whereas a second mechanism is involved in blocking the development of chimerism in these mice. Through the use of depleting mAb's and knockout mice we demonstrate that three types of recipients survived and became chimeric after being given sublethal irradiation, anti-CD154 mAb, an allogeneic bone marrow transplant and a day 0 LCMV infection: mice depleted of CD8+ T cells, CD8 knockout mice, and TCR-αβ knockout mice. Our data indicate that the mediator of bone marrow allograft destruction in LCMV-infected mice treated with costimulatory blockade is a radioresistant CD8+ NK1.1- TCRαβ+ T cell. We conclude that a non-cytopathic viral infection at the time of transplantation can prevent engraftment of allogeneic bone marrow and result in the death of sub-lethally irradiated mice treated with costimulation blockade. The abrogation of allogeneic bone marrow engraftment is mediated by a population of CD8+ NK1.1- TCRαβ+ T cells and the mediator of hypoplasia and death is viral induction of IFN-αβ.

Cardiac transplantation is governed by complex immunological mechanisms contributing to different types of allograft rejection. Early non-specific graft failure and chronic rejection (cardiac allograft vasculopathy) represent the main limitations for the recipients’ short- and long-term survival respectively. To date, the pathogenesis of both rejection types remains ill-defined. However, it is believed that they are related to an immunologically mediated potent inflammatory process, occurring whether early after transplantation (acute), or lasting for the lifetime of the graft (chronic).

The initiating mechanisms of chronic rejection in solid organ transplantation remain ill-defined. Emerging evidence sustains that graft vasculopathy is primarily driven by alloreactive CD4+ T lymphocytes sensitized by the indirect pathway of allorecognition. To date, whereas the nature of APCs involved in this particular pathway has yet to be identified, it appears challenging to speculate that recipient-derived endothelial cells (ECs) repopulating the graft may represent the main cell targets recognized by indirectly primed alloreactive CD4+ T cells to mediate the rejection of cardiac transplants. In the first part of this thesis, we specifically studied the indirect pathway of allorecognition with a transgenic mice (Marilyn mice) model that expresses a T cell receptor (TCR) transgene which recognizes the male antigen H-Y in an I-Ab-restricted fashion. Our results provide evidence that graft endothelium replacement by recipient-type cells expressing MHC Class II molecules is required for the chronic rejection of vascularized cardiac transplants mediated by indirect pathway alloreactive CD4+ T cells.

The purpose of the second part of the thesis was to investigate the potential implication of interleukin-22 (IL-22), an early phase secreted proinflammatory cytokine of the IL-10 family, in the acute rejection of cardiac allografts. IL-22 was recently described as an effector key modulator of the inflammatory process produced mainly by differentiated CD4+ T cells of the Th17 lineage. As being closely related to IL-10 and IL-17, both involved in the rejection process of vascularized heart allografts, we attempted to determine the precise role of IL-22 in this process. Experiments were conducted with a recently developed murine model deficient for the IL-22 gene (IL-22KO). The results of the second part of the thesis show that IL-22 is not an effector cytokine in cardiac allograft rejection. In contrast, as being early expressed into the allograft, likely IL-22 plays a protective role in the inflammation leading to acute cardiac rejection, probably depending on a neutrophil-related mechanism.

In conjunction with current understanding of inflammatory and antigen-specific events in allografts, overall, our results provide new insights into the mechanisms of chronic and acute cardiac rejection, thus prompting to further interrogations and appealing novel therapeutic strategies. Pharmacologic manipulation of endothelium is challenging. Given their capacity to sense and rapidly respond to the local environment, ECs are the ideal targets for rapid systemic delivery of therapeutic agents. Combination therapy is required to reduce inflammatory reaction and endothelial activation, to modulate endothelial dysfunction and promote endothelial survival. Also, given that IL-22 may alleviate tissue destruction during inflammatory responses, therapies that enhance its production and protective action in the transplanted organs seem attractive to specifically affect tissue responses, without exerting direct effects on the immune response.

Doctorat en Sciences médicales
info:eu-repo/semantics/nonPublished

Regulatory T cells (Tregs), lymphocytes that suppress immunological reactions, are of great interest for our comprehension of basic immunology and as a therapeutic agent to treat immune-mediated pathologies. Understanding the physiology of these cells will help to inform clinical strategies targeting Tregs. In order to study the homing of human Tregs, we utilised genetic engineering to drive expression of fluorescent protein in human Tregs, permitting in vivo cell tracking. We optimised a protocol for lentivirus-mediated transduction of human Tregs during in vitro expansion, to generate high yields of stably-engineered cells. After infusing labelled cells into a humanised mouse model of skin allotransplantation, we detected human Tregs within a human skin graft by PCR and visualised Tregs moving in the graft, in a live mouse, by two-photon microscopy. Through reverse genetic analyses, we explored molecular mechanisms that allow Tregs to respond adaptively to environmental cues. Neuropilin-1 (NRP1), a transmembrane co-receptor, has been implicated in the function of mouse Tregs. Tregs transduced with shRNA to knock down NRP1 were severely impaired in their capacity to suppress cell proliferation in vitro and to prolong allograft survival in a humanised mouse model. qRT-PCR analysis revealed that transcription the gene encoding the anti-inflammatory cytokine IL-10, and the autophagy-associated genes BECN1, COPS4 and MAP1LC3B, was significantly diminished in NRP1-deficient Tregs. We concluded that in human Tregs, NRP1 is necessary for suppressive function, most likely via regulation of NRP1-dependent regulation of cytokine production and metabolism. Having identified a molecular target via which Treg function might be potentiated, we explored methods to target such molecules for cell therapy applications. Tregs engineered to over-express IL-10, but not NRP1, exerted significantly enhanced suppression of cell proliferation in vitro. Thus, relatively straightforward genetic engineering, compatible with generation of therapeutic cell yields, could be exploited to improve the efficacy of Treg cellular therapy.

La transplantation d'organe est le meilleur traitement en cas de défaillance terminale d'un organe vital. Cependant, la survie sur le long terme est limitée par la perte inexorable de la fonction des greffons. Cette dernière est attribuée à l'inflammation microvasculaire (1MV) causée par la réponse anticorps contre les alloantigènes (rejet humoral chronique (RHC)). En analysant une cohorte de 129 transplantés rénaux présentant de l'1MV sur une biopsie de greffon, nous avons trouvé que, dans la moitié des cas, les lésions n'étaient pas médiées par les anticorps. Chez ces patients, des études génétiques ont révélé une prévalence plus élevée de « mismatches » entre les molécules HLA de classe 1 (HLA-1) du donneur et les « Killer-cell immunoglobulin-receptors » (K1R) inhibiteurs des NK du receveur. Nous avons émis l'hypothèse que la nature allogénique de l'endothélium du greffon pouvait créer un « pseudo-missing-self ». De ce fait, les NK du receveur, exposés à des stimuli inflammatoires, ne reçoivent plus les signaux inhibiteurs transmis par le HLA-1 de la part des cellules endothéliales du donneur. Dans un modèle de co-culture de cellules endothéliales et de NK humains, nous avons démontré que l'absence d'un ligand HLA-1 du soi sur la cellule endothéliale peut activer les NK. Cette activation dépend de la voie mTOR dans les NK, qui peut être bloquée par la rapamycine, un inhibiteur de mTORC1 disponible en clinique. Enfin, nous avons confirmé l'existence de rejets NK induit par le « missing-self » et leur sensibilité à la rapamycine dans un modèle murin de transplantation cardiaque. Notre travail identifie un nouveau type de rejet chronique, exclusivement médié par l'immunité innée, les NK, ayant le même impact délétère sur la survie des greffons que le RHC. Cependant, alors qu'il n'y a pas de traitement disponible pour le RHC, les inhibiteurs de mTOR préviennent efficacement le développement de lésions dans un modèle murin de rejet vasculaire chronique induit par le « missing self »
Organ transplantation is the best treatment for terminal organ failure. However, long-term outcome of organ transplantation remains limited by inexorable loss of graft function, which the prevalent dogma links to the microvascular inflammation (MVI) triggered by the recipient's antibody response against alloantigens (antibody-mediated chronic rejection, AMR). Analysing a cohort of 129 renal transplant patients with MVI on graft biopsy, we found that, in half of the cases, histological lesions were not mediated by antibodies. In these patients, genetic studies revealed a higher prevalence of mismatches between donor HLA-I and inhibitory Killer-cell immunoglobulin-receptors (KIR) of recipient's NK cells. We hypothesized that the allogeneic nature of graft endothelium could create a "pseudo-missing self" situation, thereby the recipient's NK cells exposed to inflammatory stimuli would not receive HLA I-mediated inhibitory signals from donor endothelial cells. In co-culture experiments with human NK cells and endothelial cells, we demonstrated that the lack of self HLA-I on endothelial cells can activate NK. This activation triggers mTOR pathway in NK, which can be blocked by rapamycin, a commercially available inhibitor of mTORC1. Finally, we confirmed the existence of missing self-induced rejection and its sensitivity to mTOR inhibition in a murine heart transplantation model. Our work identifies a new type of chronic rejection, exclusively mediated by innate NK cells, with the same detrimental impact on graft survival as AMR. However, while no therapy is available for AMR, mTOR inhibitors efficiently prevent the development of lesions in murine models of NK cell-mediated chronic vascular rejection

Allogeneic hematopoietic stem cell transplantation (allo-HCT) has been a successful cellular therapy for patients suffering from hematological malignancies for many decades; however, the beneficial effects of graft-versus-leukemia (GVL) are classically offset by graft-versus-host disease (GVHD). GVHD occurs when major and/or minor human leukocyte antigen (HLA) mismatches between donor and recipient cause rapid expansion and activation of donor effector T cells (Teffs) resulting in end organ damage to the recipient’s epithelial tissues. Given the lymphoproliferative nature of this disease, the standard treatment option is broad immunosuppression, which can result in primary disease relapse, steroid refractory GVHD, and/or opportunistic infection. A more targeted therapy that can selectively suppress GVH responses with maintained GVL responses would achieve the optimal goal of allo-HCT. Regulatory T cells (Tregs) both natural (nTregs) or induced (iTregs) could be potential cellular therapies for the treatment of GVHD, given their innate suppressive function. Initial clinical trials using nTregs have yielded positive results; however, nTreg cellular therapy has been cumbersome due to the necessity for large scale ex vivo expansion given their low yield within an apheresis product and non-specific suppression. Conversely, iTregs can be generated from naïve T cells thus decreasing ex vivo culture times and can be educated with specific antigen thus providing targeted suppression, but a consensus on their efficacy for GVHD therapy has not been reached. Therefore, we investigated the efficacy of antigen specific iTreg therapy for the prevention of GVHD while maintaining GVL responses. In Chapter 2, we evaluated the effectiveness of monoclonal HY-specific iTregs in GVHD attenuation. We chose HY as a target antigen because it is a naturally processed, ubiquitously expressed minor mismatch antigen carried by only male donors/recipients cited to increase GVHD prevalence when donor and recipient are sex-mismatched. Utilizing HY-transgenic mice in which all T cells recognize HY antigen exclusively, we generated HY specific iTregs which effectively attenuating GVHD in male, but not female recipients in three murine bone marrow transplantation (BMT) models (major mismatch, parent to F1, and miHAg mismatch). We found HY specific iTregs lost stability in female recipients but remained stable and suppressive in male recipients suggesting expression of HY antigen was required for their suppressive function and stability. GVL responses were not compromised with the addition of HY specific iTregs in recipient mice using a pre-established tumor model. Thus, HY-specific iTregs can be generated and suppress GVHD in an antigen-dependent manner while sparing the GVL effect. In Chapter 3, we extend our findings in Chapter 2, which provided proof of principle that antigen specific iTregs effectively control GVHD; however, this therapy has a limited translational potential. Therefore, we generated alloreactive CD4 and CD8 iTregs and evaluated GVHD attenuation and GVL preservation in either full or haplo-MHC mismatched BMT models. We found alloreactive CD4 iTregs significantly suppress lethal GVHD, but completely abrogated the GVL effect against aggressive tumors. Conversely, alloreactive CD8 iTregs moderately attenuated GVHD and possessed direct cytotoxicity against tumor cells. Therefore, to rescue the impaired GVL effect mediated by CD4 iTregs, we established a combinational therapy with CD8 iTregs. Indeed we found combination CD4 and CD8 iTreg therapy significantly suppressed GVHD while sparing GVL responses compared to either CD4 or CD8 singular therapy. Mechanistically, this was achieved by potent suppression of both CD4 and CD8 Teffs coupled with preserved cytolytic molecule expression by both CD8 iTregs and Teffs. Taken together, we propose antigen specific iTreg therapy can effectively attenuate GVHD while preserving GVL responses. We further uncovered unique characteristics of CD4 and CD8 iTregs that can be exploited to achieve the optimal cellular therapy following allo-HCT.

La transplantation cardiaque est aujourd'hui la seule option de traitement à long terme pour les patients souffrant d'insuffisance cardiaque terminale. Malgré des progrès considérables dans les traitements immunosuppresseurs, le rejet d'allogreffe reste une cause majeure de la perte du greffon. Dans ce domaine, des études récentes ont souligné l'importance du rejet humoral (AMR) comme un facteur contributif important à l’évolution, précoce ou tardive, de la maladie vasculaire du greffon et, in fine, à la perte de ce greffon. La pierre angulaire du diagnostic de rejet repose sur la biopsie endomyocardique (BEM) et l'évaluation histopathologique classique. Cependant, les épisodes de rejet observés sont aujourd'hui plus rares et plus complexes qu'auparavant, du fait de la présence de formes tronquées, indolentes et mixtes empêchant un diagnostic précis avec une évaluation conventionnelle. En outre, la BEM est une procédure invasive, entrainant des coûts importants, un inconfort pour le patient et un risque non négligeable de complications graves. Par conséquent, l'évaluation histologique conventionnelle ne reflète pas la complexité du rejet de greffe cardiaque et a besoin d'améliorations en termes de diagnostic. Le travail présenté dans cette thèse explore deux types de biomarqueurs, la voie mTOR, marqueur in situ, et les micro-ARNs, marqueurs circulants, qui permettraient une meilleure classification du rejet et constitueraient une aide diagnostique et/ou prédictive à la pratique clinique quotidienne lors du suivi des patients transplantés
Cardiac transplantation is currently the only option for long-term treatment for patients with terminal heart failure. Despite considerable advances in immunosuppressive therapy, allograft rejection remains a major cause of graft loss. In this regard, recent studies have highlighted the importance of antibody-mediated rejection (AMR) as an important contributory factor in the evolution of vascular graft disease and, ultimately, graft loss. The cornerstone of the rejection diagnosis is based on endomyocardial biopsy (EMB) and the classical histopathological evaluation. However, rejection episodes observed today are becoming scarce and more complex than before, due to the presence of truncated, indolent and mixed forms preventing an accurate diagnosis with a conventional assessment. In addition, the biopsy is an invasive procedure, resulting in significant costs, discomfort for the patient and a significant risk of serious complications. Therefore, conventional histological assessment does not reflect the complexity of cardiac transplant rejection and needs improvement in terms of diagnosis. The work presented in this thesis explores two types of biomarkers, the mTOR pathway, an in situ marker, and the micro-RNAs, circulating markers that would allow a better classification of rejection and provide diagnosis and/or predictive help to daily clinical practice during the monitoring of transplant patients

La greffe cardiaque est le traitement ultime de l’insuffisance cardiaque. Le rejet aigu pose plusieurs problématiques, en particulier sa survenue imprévisible même sous traitement immunosuppresseur, et un diagnostic histologique qui nécessite des biopsies endomyocardiques (BEM) invasives répétées, et qui souffre de nombreuses limites. Le besoin de critères diagnostiques et prédictifs, idéalement non invasifs, nous a conduits à étudier le rejet aigu de greffe cardiaque sur le plan moléculaire. Nous avons caractérisé les profils d’expression génique (PEG) myocardiques et sanguins lors de différentes phases du rejet cellulaire (RC) et du rejet médié par les anticorps (RMA), par analyse sans a priori des transcriptomes sur puce à ADN. Par une première étude des PEG myocardiques menée sur une collection historique de BEM, nous avons montré la modification des PEG tissulaires lors du RC. Pour le même grade histologique, deux profils de RC aux degrés d’activation immunitaire différents ont été identifiés. De plus, les PEG myocardiques étaient modifiés dès un mois avant la survenue d’un RC, quand l’analyse histologique ne montrait encore aucune anomalie. Par une seconde étude conduite sur une collection prospective de BEM et échantillons sanguins, nous avons confirmé les résultats de la première étude, et de plus montré l’existence de modulations des PEG également dans le sang périphérique, aussi bien pendant un épisode de RC qu’un mois avant. Enfin pour la première fois la modulation tissulaire et périphérique des PEG a été montrée dans le RMA en transplantation cardiaque. L’existence de voies modulées dans les deux types de rejet devrait conduire à la recherche de biomarqueurs
Heart transplantation is the last treatment in case of terminal heart failure. Acute rejection after heart transplantation raises several issues due to its occurrence despite immunosuppressive therapies and the requirement of invasive and repeated endomyocardial biopsies (EMB) that have several histological grading limitations. The need of non-invasive diagnostic and predictive criteria led us to study the acute rejection of cardiac allograft using a molecular approach. We characterized myocardial and peripheral blood gene expression profiles (GEP) during acute cellular rejection (CR) and antibody-mediated rejection (AMR) by mean of microarray analyses. By a retrospective study conducted on a historical EMB collection, we first showed a strong immunologic modulation during CR. For the same CR histological grading, two transcriptional profiles were identified according to the inflammation level. Moreover, myocardial GEP modifications were observed one month before the occurrence of CR, while histological characteristics showed no abnormality. A second study conducted on a prospective collection of both EMB and peripheral blood samples confirmed the results obtained on EMB and showed peripheral blood GEP modulations during both CR and even one month earlier. Finally, we have also shown for the first time in heart transplantation, myocardial and peripheral GEP modulations in AMR. Identification of modulated pathways in both types of rejection should allow for the determination of rejection biomarkers

A partir da década de 60, com a utilização do transplante renal em larga escala como terapia substitutiva para pacientes com falência do órgão, surgiu a preocupação quanto ao desenvolvimento do processo de rejeição do enxerto. Tal intercorrência, em geral, cursa com sinais e sintomas clínicos apenas quando o evento está bem estabelecido, ou mesmo quando lesões irreversíveis já se instalaram. Assim, é fundamental um acompanhamento rigoroso, visando detectar os casos subclínicos. O presente trabalho, a fim de fornecer novas ferramentas que auxiliem o diagnóstico precoce de rejeição do enxerto, avaliou a expressão imuno-histoquímica dos anticorpos CD3, CD5, CD20, CD68, CD25, FoxP3 e C4d em biópsias renais realizadas entre os anos de 2007 e 2009 em pacientes transplantados acompanhados pelo Serviço de Nefrologia do Hospital Universitário Pedro Ernesto, UERJ - RJ, correlacionando os resultados obtidos com o diagnóstico histológico. Para tal, as biópsias foram reavaliadas por três médicos patologistas que as classificaram, segundo Critérios de Banff 2007, quanto à presença ou não de rejeição do enxerto e seu tipo, aguda ou crônica. A partir de então, os blocos de parafina foram processados pela técnica Tissue Microarray for all (Pires, ARC. e cols.) e submetidos à imuno-histoquímica. A positividade dos marcadores foi avaliada e graduada e os resultados encontrados foram correlacionados, em um primeiro momento, com a presença ou ausência de rejeição. Posteriormente, os casos com diagnóstico histológico de rejeição tiveram seu perfil imuno-histoquímico analisado em função da positividade para C4d, marcador definidor de rejeição humoral. Neste momento, buscou-se averiguar se os anticorpos estudados seriam úteis em detectar, neste grupo, rejeição humoral e celular. Após a análise estatística, realizada pelo Teste Exato de Fisher, pode-se, então, concluir que o comportamento do marcador CD3 é capaz de inferir a presença de rejeição e que os anticorpos CD5 e CD25 permitem sugerir rejeição celular e humoral, respectivamente. Foi observado também que casos sem diagnóstico histológico de rejeição podem apresentar marcação para C4d em mais de 10% de seus capilares peritubulares.
From the 60's, with the use of renal transplantation on a large scale as replacement therapy for patients with organ failure, came out the concern about the development process of graft rejection. This intercurrence, generally, evolves with clinical signs and symptoms only when the event is well established, or even when irreversible damage has already been installed. So, is essential a close monitoring, looking forward to detect subclinical cases. The present work, in order to provide new tools that help in the early diagnosis of rejection of the graft, evaluated the immunohistochemical expression of CD3, CD5, CD20, CD68, CD25, FoxP3 and C4d in renal biopsies performed between the years 2007 and 2009 in transplanted patients accompanied by the Department of Nephrology of Pedro Ernesto University Hospital, UERJ - RJ, correlating the results with the histological diagnosis. To this, the biopsies were evaluated by three pathologists who classified them, according to Banff 2007 Criteria, for the presence or absence of graft rejection and its type, acute or chronic. Thereafter, the paraffin blocks were processed by Tissue Microarray for all technique (Pires, ARC. & cols.) and submitted to immunohistochemistry. The positivity of the markers was evaluated and graded and the results were correlated, at first, with the presence or absence of rejection. Later, cases with histological diagnosis of rejection had their immunohistochemical profile considered according to the positivity for C4d, a defining marker of humoral rejection. At this point, we sought to determine whether the antibodies would be useful in detecting, in this studied group, humoral and cellular rejection. After statistical analysis, performed by Fisher's Exact Test, it could be, therefore, concluded that the behavior of the CD3 marker is able to infer the presence of rejection and that CD5 and CD25 antibodies may suggest cellular and humoral rejection, respectively. It was also observed that cases without histological diagnosis of rejection may have markings for C4d in more than 10% of their peritubular capillaries.

Summary

Immune homeostasis relies on a subtle balance between fight towards pathogens and inhibitory mechanisms that prevent inappropriate responses against self and environmental antigens (allergy). Regulatory T (Treg) cells play a central role in this balance. Optimizing Treg effects represents a promising approach for new stratetiges aiming to induce or restore tolerance against allo or self antigens. The first part of this work demonstrates that CD4+ lymphocytes that secrete IL-17A (Th17) promote allograft rejection in a murin model of skin transplantation with minor antigen disparities. Interestingly, Treg cells strengthen rather than inhibit Th17 effector mechanisms in this model. Indeed, we found that in vivo Treg depletion prevented IL-17 production by recipient T cells. An adoptive cotransfer of Treg with naive monospecific antidonor T cells in lymphopenic hosts biased the immune response towards a dominant Th17 phenotype. Finally, we observed that IL-6 was central for balancing Treg and Th17 cells as demonstrated by the prevention of Th17 differentiation, the enhanced Treg/Th17 ratio, and rejection blockade in the absence of IL-6. In conclusion, the ability of Treg to promote a Th17 pathway of rejection we described should be considered as a potential drawback of Treg-based cell therapy.

Based on the hypothesis that Treg promote Th17 immune response, we tested the effect of IL-17A neutralization in a model in which long-term skin allograft survival depends on a transient in vivo Treg expansion induced by exogenous IL-2. As expected, IL-2 administration prevented rejection of MHC class II disparate skin allografts. Surprisingly this treatment was inefficient in IL17A-/- recipients. We attested that IL-17A was not required for IL-2-mediated Treg expansion, recruitment or suppressive capacities. Instead, IL-17A prevented allograft rejection by inhibiting Th1 alloreactivity independently of Treg. Indeed, T-bet expression of naïve alloreactive CD4+ T cells and the subsequent Th1 immune response was significantly enhanced in IL-17A deficient mice. Our results illustrate, to our knowledge, for the first time a protective role of IL-17A in CD4+-mediated allograft rejection process.

In the last part of this work, we used the same mouse model of MHC class II-mismatched skin grafts in which long-term acceptance is achieved by a short-term administration of exogenous IL-2. We first confirmed that Tregs play a central role in preventing skin graft rejection as attested by the prompt donor skin destruction occuring after Treg cell depletion.

In the context of IL-2-mediated anti-rejection therapy, concomitant costimulatory blockade with CTLA4-Ig paradoxically restored skin allograft rejection and Th1 alloreactivity indicating that Treg-mediated suppresion absolutely required CD28-B7 or CTLA4/B7 interactions. Further experiments showed that CTLA4-Ig inhibited IL-2-driven Treg expansion, and prevented in particular the occurrence of ICOS+ Treg endowed with potent suppressive capacities. Restoring CD28 signaling was sufficient to counteract the deleterious effect of CTLA4-Ig on Treg expansion and functionality, in keeping with the hypothesis that costimulatory blockade inhibits Treg expansion and function by limiting the delivery of essential CD28-dependent signals. Inhibition of regulatory T cell function should therefore be taken into account when designing tolerance protocols based on costimulatory blockade.

RÉSUMÉ

Le bon fonctionnement du système immunitaire résulte d’un équilibre entre les réponses immunes « effectrices » qui luttent contre les pathogènes et des mécanismes « régulateurs » permettant de les contrôler. Parmi ces mécanismes inhibiteurs, les lymphocytes T régulateurs (Treg) jouent un rôle crucial. En empêchant le débordement des réponses effectrices, ils préviennent l’apparition des allergies et des maladies auto-immunes ou inflammatoires. Dès lors, il est aisé d’imaginer le potentiel thérapeutique de ces cellules pour contrecarrer les phénomènes autoimmuns ou les réponses allogéniques responsables du rejet en transplantation. C’est donc l’étude des Treg chez la souris qui se trouve au centre des nos préoccupations dans ce travail.

Dans la première partie, nous avons démontré le rôle des lymphocytes CD4+ sécréteurs d’IL-17A (Th17) dans le rejet de greffe de peau présentant une disparité d’antigène mineur de transplantation. Dans ce modèle de rejet « Th17 », les données indiquent que, contrairement aux lignées Th1 et Th2, la réponse Th17 est favorisée par les Treg renversant ainsi le paradigme absolu du « Treg inhibiteur ». En effet, la déplétion des Treg dans notre modèle abolit l’expression des gènes caractéristiques de la voie Th17. De plus, dans un système de transfert adoptif chez la souris lymphopénique, l’ajout de Treg à une population T CD4+ effectrice naïve favorise leur différenciation en Th17. Enfin, en invalidant le gène de l’IL-6 dans notre combinaison allogénique mineure, nous avons mis en évidence la place importante de cette cytokine dans le rejet Th17 ainsi que dans la balance Th17/Treg en alloimmunité.

En partant du postulat que les Treg favorisent les réponses Th17, nous avons étudié l’impact de la déficience en IL-17A dans un modèle de greffe de peau réalisée en présence de quatités acrues de Treg. Pour cela, nous avons utilisé un modèle de rejet induit par une disparité isolée du CMH II au cours duquel les Treg sont amplifiés par l’injection d’IL-2 exogène durant les trois premiers jours de greffe. Dans ce système, l’expansion transitoire des Treg chez le receveur « sauvage » bloque le rejet dans 75% des cas jusqu’au jour 60 après la greffe sans le moindre traitement immunosuppresseur. Contre toute attente, l’absence d’IL-17A dans ce système restaure le rejet (receveurs IL-17A-/-). Nous avons démontré que l’IL-17A n’est pas requise pour l’expansion, la migration ou la fonction des Treg amplifiés par l’IL-2. En fait, les résultats suggèrent que l’IL-17A bloque le rejet en inhibant la réponse Th1 indépendamment des Treg. Ce point est appuyé par l’exacerbation de la voie Th1 chez le receveur IL-17A-/- et l’inhibition de l’expression de T-bet sous l’influence de l’IL-17A en culture mixte lymphocytaire. Paradoxalement, cette partie du travail rapporte donc un effet protecteur de l’IL-17A illustrant toute la complexité des rôles joués par cette cytokine.

La dernière partie du travail utilise le même modèle de greffe de peau allogénique (disparité du CMH II) dans lequel le rejet aigu est bloqué par l’expansion in vivo des Treg induite par l’IL-2 exogène. Nous avons confirmé que l’acceptation à long terme des greffons repose sur les propriétés inhibitrices des Treg amplifiés. Cette inhibition du rejet nécessite impérativement l’intégrité des interactions survenant entre les Treg et les cellules présentatrices d’antigènes du receveur via les molécules B7/CD28. L’ajout de CTLA4-Ig, un immunosuppresseur bloquant les interactions de ces molécules, conduit invariablement à l’accélération paradoxale du rejet. Cet effet pro-inflammatoire du CTLA4-Ig, s’explique par une action délétère sur la survie et la qualité des Treg. En conclusion, les données expérimentales obtenues dans ce dernier volet démontrent l’effet délétère potentiel de ce type de traitement dans les protocoles d’induction de tolérance basé sur l’emploi des Treg.

Doctorat en sciences médicales
info:eu-repo/semantics/nonPublished

Estudos com células tronco mesenquimais (CTm) têm despertado grande interesse devido a seu promissor potencial terapêutico e representam uma alternativa para o tratamento de diversas patologias em diferentes órgãos, inclusive em transplante renal. A rejeição crônica é um dos maiores desafios no transplante tardio e se caracteriza por perda progressiva da função renal causado pela intensa fibrogênese no aloenxerto. Os tratamentos convencionais com imunossupressores, apesar de reduzirem significativamente as crises de rejeição aguda, não interferem na sobrevida do enxerto a longo prazo. A compreensão dos processos fisiopatológicos da doença depende de seu estudo em modelos experimentais, que são de grande importância pois também propiciam uma melhor compreensão dos possíveis tratamentos. O presente estudo teve como objetivo analisar a terapia com células-tronco mesenquimais derivadas de tecido adiposo (CTmTA) no modelo experimental de transplante renal em ratos, para estudar seu efeito na rejeição crônica e avaliar seu potencial efeito imunomodulador. O modelo foi estabelecido com ratos das linhagens isogênicas Fisher (doador) e Lewis (receptor) e os animais transplantados foram divididos em três grupos: ISO (transplante isogênico de Lewis para Lewis, n=6), ALO (transplante alogênico de Fisher para Lewis, n=6) e ALO+CTmTA (transplante alogênico, tratado com CTmTA, n=6). As CTmTA foram caracterizadas por aderência ao plástico, diferenciação nas linhagens adipogênica, condrogênicas e osteogênicas e por citometria de fluxo. Foram inoculadas 1 x 106 células na região subcapsular renal no dia da realização da nefrectomia unilateral direita (10 dias pós-transplante). Após 6 meses foram realizadas análises dos parâmetros clínicos e laboratoriais, além de análise histológica, imunohistoquímica e PCR em tempo real. As CTmTA foram eficientes em prevenir significativamente a elevação da ureia e da creatinina séricas, manter clearence de creatinina em níveis normais, e prevenir a elevação da fração de excreção de Na+ e K+. Além disso, impediram o desenvolvimento de proteinúria e da hipertensão arterial. A análise histológica mostrou uma redução significativa do infiltrado inflamatório de macrófagos e linfócitos T, além de uma diminuição da fibrose intersticial no grupo ALO+CTmTA. O tratamento com CTmTA reduziu significativamente a expressão relativa dos fatores e citocinas pró-inflamatórios tais como INF-y, TNF-alfa, IL1beta e IL-6, além de aumento importante na expressão de IL-4 e IL-10, conhecidas por seu potencial antiinflamatório. Em conclusão, o tratamento com ADMSC em um modelo experimental de transplante renal pode trazer uma nova abordagem terapêutica para controle da rejeição crônica do enxerto. A aparente modulação da resposta imune observada neste trabalho, pode estar associada a uma possível polarização de macrófagos e células T. Outros estudos pré-clínicos e clínicos são necessários para confirmar nossos resultados
Studies involving mesenchymal stem cells (MSCs) have aroused great interest due to their promising therapeutic potential representing an alternative for the treatment of several pathologies in different organs, including renal transplantation. Chronic rejection is one of the major challenges in late transplantation and is characterized by progressive loss of renal function caused by intense fibrogenesis in the allograft. Conventional immunosuppressive treatments, while significantly reducing acute rejection crises, do not interfere with long-term graft survival. Animal model of kidney transplantation can provide a better understanding of the pathophysiological processes and bring a new path to treat chronic rejection. The aim of this project was to analyze the therapy with mesenchymal stem cells derived from adipose tissue (ADMSCs) in the experimental model of kidney transplantation in rats, focus on chronic rejection and evaluate its potential immunomodulatory effect. The model was established with rats of isogenic strains Fisher (donor) and Lewis (recipient), and the transplanted animals were divided into three groups: ISO (isogenic transplantation from Lewis to Lewis, n = 6), ALO (allogenic transplant from Fisher to Lewis, n = 6) and ALO + ADMSCs (allogenic transplantation, treated with ADMSCs, n = 6). ADMSCs were characterized by adhesion to plastic, differentiation in adipogenic, condrogenic and osteogenic lines and by flow cytometry. One million of cells were inoculated under the renal capsule on the day of the right unilateral nephrectomy (10 days after transplantation). After 6 months, clinical and laboratory parameters were analyzed, as well as histological analysis, immunohistochemistry and real-time PCR. ADMSCs were effective in preventing elevation of serum urea and creatinine, elevation of the Na + and K + excretion fraction as well as maintained creatinine clearence at normal levels. Furthermore, the treatment also prevented the development of proteinuria and preserved blood pressure. Histological analysis showed a significant reduction of macrophages and T cells infiltrate, associated to a decreased of interstitial fibrosis in the ALO + ADMSCs group. In the presence of ADMSCs, there was a significant decrease in the relative expression of INF-y, TNF-alpha, IL1beta and IL-6 factors and pro-inflammatory cytokines, as well as a significant increase in the relative expression of anti-inflammatory cytokines as IL-4 and IL-10. In conclusion, treatment with ADMSC in a transplantation model could open a new approach to control chronic rejection. This apparent modulation of the immune response may be associated with a possible polarization of macrophages and T cells. Further pre-clinical and clinical studies are needed to confirm our findings

Le rejet d’allogreffe dépend de la reconnaissance d’antigènes d’histocompatibilité étrangers par le système immunitaire du receveur. En l'absence de thérapies immunosuppressives, la réaction inflammatoire éventuelle conduit à la destruction rapide du tissu transplanté. Le rôle critique joué par les lymphocytes T CD4+ dans le rejet aigu d'allogreffe est bien établi. Cependant, les contributions respectives des lymphocytes CD4+ Th1 et Th2 dans la réaction de rejet sont controversées. Alors que le rôle des cellules Th1 dans la pathogénèse du rejet est bien établi, l'hypothèse que les cellules Th2 favorisent l'acceptation de la greffe est invalide puisque ces cellules sont capables de déclencher des voies alternatives de rejet. En effet, la fonction effectrice des lymphocytes Th2 a été démontrée dans beaucoup de modèles de rejet de greffe ou de tumeur, et dans la maladie du greffon contre l'hôte. Les caractéristiques principales du rejet de type Th2 sont sa dépendance envers la production d'IL-4 et d'IL-5, le recrutement d'éosinophiles au site du rejet, et son inhibition par les lymphocytes T CD8+ alloréactifs. Les éosinophiles activés exercent leur activité cytotoxique par la libération de plusieurs molécules cytotoxiques comme l’EDN, l’ECP, la MBP et l’EPO. Ces molécules sont probablement responsables de la capacité des éosinophies à affecter la perméabilité vasculaire et à induire des dégâts tissulaires dans les organes rejetés.

L'interleukine 9 (IL-9) est une cytokine produite par les lymphocytes T qui joue un rôle important dans les voies effectrices Th2. Dans la littérature, l’IL-9 est fortement associée au développement de l’éosinophilie tissulaire. Dans notre première étude, nous avons analysé le rôle joué par l'IL-9 dans le rejet d'allogreffe bm12 par des souris B6 (pour C57BL/6), un modèle dans le lequel une simple disparité au niveau de la molécule du CMH de classe II favorise une réaction inflammatoire de type Th2. Dans ce modèle, de faible alloantigénicité, les greffes cardiaques bm12 survivent presque indéfiniment dans les receveurs B6 (>60 jours). Nos expériences ont été conçues afin de savoir si l’expression de l’IL-9 au niveau de la greffe pouvait modifier la survie de greffes cardiaques exprimant les alloantigènes bm12. Nous avons ainsi montré que la production locale d’IL-9 induit le rejet des allogreffes cardiaques exprimant l’alloantigène I-Abm12 (survie <30jours). Aucun des organes transgéniques pour l’IL-9 n’a survécu plus de 30 jours alors que des greffes non transgéniques ne furent pas rejetées (>50 jours). L’analyse histologique des allogreffes cardiaques transgéniques pour l’IL-9 montre une infiltration cellulaire dense du myocarde. La composante principale de cet infiltrat est la présence de nombreux éosinophiles.

Pour étudier la contribution des cytokines de type Th2, comme l’IL-4 et l’IL-5, dans le rejet des cœurs transgéniques pour l’IL-9, nous avons sélectivement bloqué ces cytokines lors du processus de rejet. Le traitement avec des anticorps neutralisant l’IL-4 bloque complètement le rejet induit par l’IL-9 et permet la survie à long terme des allogreffes cardiaques. Au point de vue de l’histologie ces greffes ne montrent ni infiltration leucocytaire ni artériopathie. Afin de déterminer si l’infiltration éosinophilique induite par l’IL-9 provient de l’activité directe de l’IL-9 ou est le résultat de la sécrétion d’IL-5, un traitement avec un anticorps anti-IL-5 a été appliqué aux receveurs d'allogreffe cardiaque. Ce traitement augmente la survie de la majorité des allogreffes et modifie de manière marquée la composition de l’infiltrat cellulaire en prévenant le recrutement des éosinophiles. De manière intéressante, les cœurs transgéniques pour l’IL-9 qui survivent indéfiniment après le traitement anti-IL-5 arborent une importante fibrose.

A la différence du cœur bm12, la peau bm12 greffée sur un receveur B6 subit un rejet rapide et l'histologie des greffes rejetées révèle la présence d'infiltrats denses à éosinophiles. Notre laboratoire a montré que ce processus de rejet est dirigé par les lymphocytes T CD4+ alloréactifs et que les souris B6 déficientes pour l'IL-5 et la voie de cytotoxicité Fas/Fas-L sont incapables de rejeter des peaux bm12. Nos premiers résultats laissaient supposer un rôle pour l'IL-9 dans notre modèle de rejet de greffes en disparité des molécules du CMH de classe II: premièrement, nous avions observé la production d'IL-9 par les lymphocytes T de type Th2 alloréactifs et deuxièmement, l'ARNm d'IL-9 était fortement exprimé au niveau des allogreffes de peaux rejetées. C’est pourquoi, la survie de peaux bm12, déficientes pour la molécule Fas, greffées sur des receveurs B6 déficients pour l'IL-9 (B6.IL-9-/-) a été comparée avec celle de peaux transplantées sur des receveurs B6. Nous avons montré que, comme les souris B6 normales, les animaux B6.IL-9-/- rejettent leur greffe dans les 15 jours. Donc, contrairement à l'IL-5, l'IL-9 n'est pas essentielle pour le rejet de peau dirigé par les cellules T CD4+ de type Th2 dans notre modèle de disparité des molécules du CMH de classe II.

Néanmoins, les allogreffes de peaux, dans notre modèle de disparité des molécules du CMH de classe II, contiennent moins d’éosinophiles lorsqu’elles sont rejetées par des receveurs déficients pour la synthèse d’IL-9 (IL-9-/-). En plus du modèle bm12, nous avons également observé un rôle de l’IL-9 dans un autre modèle de rejet Th2. Il a été montré par notre laboratoire que le rejet d’allogreffes cardiaques Balb/c complètement incompatibles par des souris receveuses B6.CD8-/- est caractérisé par le recrutement d’éosinophiles dans l’organe rejeté (106). Dans celui-ci, l’ARNm de l’IL-9 est présent pendant le rejet, de même que l’IL-4 et l’IL-5 et les greffes rejetées par des receveurs IL-9-/- contiennent moins d’éosinophiles par rapport à des receveurs contrôles. Les mécanismes par lesquels l’IL-9 induit le recrutement des éosinophiles ne sont pas complètement connus.

L’IL-5 est considérée comme la cytokine clé pour le développement de l’éosinophilie. De plus, le rejet aigu des cœurs transgéniques pour l’IL-9 est caractérisé par une infiltration massive d'éosinophiles et est inhibé lors de la neutralisation de l'IL-5. Nous avons entrepris la seconde étude pour investiguer le lien fonctionnel entre l’IL-9 et l’IL-5 dans le rejet d’allogreffe, ce qui permettra de mieux comprendre le recrutement des éosinophiles par l’IL-9.

Bien que le rejet ne soit pas inhibé par le manque d’IL-9, les allogreffes rejetées par les souris déficientes en IL-9 contiennent moins d’éosinophiles par rapport à des souris contrôles et présentent une production plus faible d’IL-5 par les cellules T alloréactives. De manière intéressante, la production optimale d’IL-5 après une stimulation allogénique requiert un récepteur à l’IL-9 (IL-9R) fonctionnel sur les cellules répondeuses. De plus, l’infiltration d’éosinophiles induite par l’IL-9 est absente dans des peaux transplantées sur des receveurs déficients pour le récepteur de l’IL-9. Finalement, la production d’IL-5 par des cellules T CD4+ stimulées par l’anti-CD3 est abolie par la neutralisation de l’IL-9.

En conclusion, nous pouvons dire que l'IL-9 est capable d'induire un rejet de type Th2, caractérisé par une forte infiltration d’éosinophiles et une dépendance à l'IL-5 et à l'IL-4. Notre étude montre également que l’IL-9 peut agir directement sur les cellules T CD4+ pour induire leur capacité à sécréter de l’IL-5. Cependant, l’IL-9 n’est pas indispensable au processus de rejet Th2 et il est probable que lorsque l’IL-9 est bloquée d'autres cytokines soient capables de compenser son absence. Notre étude permet une meilleure compréhension des voies complexes du recrutement des éosinophiles.

Doctorat en sciences biomédicales
info:eu-repo/semantics/nonPublished

The long-term survival of heart transplants is limited by the development of allograft vasculopathy (AV), a vascular pathology that develops in spite of the use of modern immunosuppressive therapies. Although it is widely accepted that T cells play a major role in the development of AV, the contribution of B cells and antibody has been less well characterized. A fully MHC-mismatched cell transfer model was used to mimic the antigenic stimulus of a cardiac graft, we examined the production of antibody under conditions of clinically relevant immunosuppression in the form of the calcineurin inhibitor cyclosporine A (CyA). Anti-donor antibody with the capacity to mediate complement-dependent cytotoxicity of donor strain cells, but not third-party cells, developed in the presence of two different doses of CyA (30 mg/kg and 50 mg/kg). When this antibody was passively transferred into immunodeficient B6.RAG1-/- abdominal aortic graft recipients, the antibody alone had the capacity to mediate formation of a neointimal lesion and induce the loss of medial smooth muscle cells. These are two hallmark characteristics of AV in this animal model. A wild-type model, where BALB/c grafts were transplanted into B6 recipients and received daily CyA immunosuppression was used to test the de novo antibody response to the transplant itself. Again, anti-donor antibody was produced with the capacity to mediate complement-dependent cytotoxicity of donor cells. In addition, grafts showed evidence of C4d deposition in the medial area, indicating that area as a sit of antibody binding and activation of the classical complement cascade. The presence of anti-donor antibody has been demonstrated to correlate with poorer graft outcome and a higher risk of developing AV in patients. Examination of human epicardial coronary artery tissue from patients with cardiac transplants demonstrated the presence in the adventitia of ectopic lymphoid structures (ELS) containing CD20+ B cells, plasma cells, IgM, and IgG. These findings illustrate active, antibody-producing ELS in close proximity to the vessels developing AV. Of note was the finding of CD20+CD27+ memory B cells in these ectopic lymphoid structures. Memory B cells are rapidly re-activated following exposure to their cognate antigen and easily differentiate into plasma cells. Taken together, these data suggest that memory B cells and antibody may be contributing to long-term allograft rejection and therapeutic options should be considered to target these immune mechanisms.

Trabalho final de mestrado integrado em Medicina área científica de Cirurgia Cardiotorácica e Anatomia Patológica, apresentado á Faculdade de Medicina da Universidade de Coimbra
Introdução e objetivos: O impacto da rejeição celular aguda durante os primeiros anos após o transplante cardíaco na sobrevida a longo prazo ainda não está bem estabelecido, assim como o seu papel no desenvolvimento da doença vascular do enxerto. Os novos imunossupressores conduziram a uma diminuição da incidência da rejeição celular aguda, mas consequentemente levaram a um aumento do risco de infeções e tumores. O objetivo do nosso trabalho foi analisar o impacto da rejeição celular na sobrevida e a ocorrência de neoplasias, infeções e doença vascular do enxerto em doentes selecionados. Métodos: De novembro de 2003 a maio de 2013, 218 doentes foram submetidos a transplante cardíaco. Doentes com menos de 18 anos, sujeitos a outro transplante de órgão prévio ao transplante cardíaco e recetores que faleceram nos primeiros 14 dias após a cirurgia devido a falência do enxerto, foram excluídos. Transplantados com pelo menos um episódio de rejeição celular aguda classificada como 2R ou 3R (Grupo A n=47) foram comparados com recetores livres de episódios de rejeição ou com episódios de rejeição classificados como 1R nos primeiros 3 anos após transplante cardíaco (Grupo B n=171). Os critérios de seleção dos dadores e recetores foram idênticos em ambos os grupos. Resultados: A incidência da rejeição celular aguda foi mais elevada nos primeiros 6 meses após transplante cardíaco (P<0.001). Não foram encontradas diferenças estatisticamente significativas na sobrevida a longo prazo (P=0.101) ou na incidência da doença vascular do enxerto (P=0.144) entre ambos os grupos. No entanto, verificámos uma ligeira tendência para a diminuição da sobrevida a longo prazo (61.7 ± 7.3% vs 77.1 ± 3.7%) e sobrevida livre de doença vascular do enxerto (75.9 ± 6.6% vs 86.0 ± 3.5%) no grupo A. As neoplasias de novo tiveram uma maior incidência no grupo B (P=0.026) enquanto as infeções foram mais frequentes no grupo A (P=0.036). Conclusão: A taxa da rejeição celular aguda na nossa população de estudo verificou-se ser baixa e a maioria dos episódios ocorreram nos primeiros 6 meses após o transplante. O tratamento imunossupressor associado talvez a um estado sobre-terapêutico podem potenciar o aumento da incidência de tumores. Este estudo sugere-nos ainda que pacientes que sofreram de episódios de rejeição celular aguda nos primeiros 3 anos após o transplante têm uma maior tendência a sofrer de doença vascular do enxerto e a uma menor sobrevida a longo prazo, no entanto sem significância estatística.
Background The impact of acute cellular rejection (ACR) on long-term survival during the first years after heart transplant has not yet been established, as well as its role on cardiac allograft vasculopathy (CAV). New immunosuppressors have led to a decline of the incidence of ACR and led to increased risk of infections and tumors. We analysed the impact of ACR on long-term survival and considered the occurrence of malignancy, infections and cardiac allograft vasculopathy in the selected patients. Methods Between November 2003 and May 2013, 218 heart transplants were performed. Patients under 18-years old, patients undergoing organ transplantation before heart transplant and recipients who died within the first 14 days after heart transplant (HT) due to graft failure, were excluded. Recipients with at least one episode of ACR event graded as 2R or 3R (Group A n=47) were compared with recipients free of rejection events or with an ACR event graded minor than 2R in the first 3 years after heart transplantation (Group B n=171). Patient/donor criteria were selected as identical in both groups. Results Incidence of ACR was higher in the first 6 months after heart transplantation (P < 0.001). There was no significant statistical difference in long-term survival (P =0.101) or incidence of CAV (P=0.144) between the two groups. A slightly tendency for a lower 7 long-term survival (61.7 ± 7.3% vs 77.1 ± 3.7%) and survival free of CAV (75.9 ± 6.6% vs 86 ± 3.5%) was verified in Group A. Malignancy de novo had an higher incidence in Group B (P=0.026) while infections (P=0.036) were more frequent in Group A. Conclusion With this study, we verified that we have a small rate of ACR and mostly occurs in the first 6 months. The effective immunosuppression regimen maybe together with over-immunosuppression may lead to a higher incidence of tumors. This study also suggests that recipients with ACR events are more likely to suffer from CAV and to have a lower long-term survival however with out statistical significance.

Indiana University-Purdue University Indianapolis (IUPUI)
Human cord blood (CB) derived circulating endothelial colony forming cells (ECFCs) display a hierarchy of clonogenic proliferative potential and possess de novo vessel forming ability upon implantation in immunodeficient mice. Since survival of ECFC post-implantation is a critical variable that limits in vivo vasculogenesis, we tested the hypothesis that activation of Notch signaling or co-implantation of ECFC with human platelet lysate (HPL) would enhance cultured ECFC vasculogenic abilities in vitro and in vivo. Co-implantation of ECFCs with Notch ligand Delta-like 1 (DL1) expressing OP9 stromal cells (OP9-DL1) decreased apoptosis of ECFC in vitro and increased vasculogenesis of ECFC in vivo. The co-culture of ECFC with HPL diminished apoptosis of ECFC by altering the expression of pro-survival molecules (pAkt, pBad and Bcl-xL) in vitro and increased vasculogenesis of human EC-derived vessels both in vitro and in vivo. Thus, activation of the Notch pathway by OP9-DL1 stromal cells or co-implantation of ECFC with HPL enhances vasculogenesis and augments blood vessel formation by diminishing apoptosis of the implanted ECFC. The results from this study will provide critical information for the development of a cell therapy for limb and organ re-vascularization that can be applied to recovery of ischemic tissues in human subjects.

Indiana University-Purdue University Indianapolis (IUPUI)
Solid organ transplantation is limited by available donor allografts. Pig to human transplantation, xenotransplantation, could potentially solve this problem if physiologic and immunologic incompatibilities are overcome. Genetic modifications of pigs have proven valuable in the study of xenotransplantation by improving pig to human compatibility. More genetic targets must be identified for clinical success. First, this study examines platelet homeostasis incompatibilities leading to acute thrombocytopenia in liver xenotransplantation. Mechanisms for xenogeneic thrombocytopenia were evaluated using liver macrophages, Kupffer cells, leading to identification of CD18, beta-2 integrin, as a potential target for modification. When disruption of CD18 was accomplished, human platelet binding and clearance by pig Kupffer cells was inhibited. Further, human and pig platelet surface carbohydrates were examined demonstrating significant differences in carbohydrates known to be involved with platelet homeostasis. Carbohydrate recognition domains of receptors responsible for platelet clearance Macrophage antigen complex-1 (CD11b/CD18) and Asialoglycoprotein receptor 1 in pigs were found to be different from those in humans, further supporting the involvement of platelet surface carbohydrate differences in xenogeneic thrombocytopenia. Second, immunologic incompatibilities due to antibody recognition of antigens resulting in antibody-mediated rejection were studied. Identification of relevant targets was systematically approached through evaluation of a known xenoantigenic protein fibronectin from genetically modified pigs. N-Glycolylneuraminic acid, a sialic acid not found in humans, was expressed on pig fibronectin and was identified as an antigenic epitope recognized by human IgG. These studies have provided further insight into xenogeneic thrombocytopenia and antibody-mediated rejection, and have identified potential targets to improve pig to human transplant compatibility.

Since its beginning, graft rejection remains the key problem of solid organ transplantation. This reaction of the recipient's immune system against mismatched antigens of the transplanted organ causes graft damage and consequently loss of its function. Rejection involves cellular (lymphocyte mediated) and humoral (antibody mediated) mechanisms. Among the genetic factors which may have a prognostic value in rejection risk evaluation are the Human Leukocyte Antigens (HLA) genotype, the Killer Immunoglobuline-like Receptor (KIR) gene repertoir, cytokine and other gene polymorphisms. These factors could be screened for before transplantation to find the best possible combination of genetic characteristics of the donor and recipient and to reveal patients with "risky" genotypes, who may need more intensive immunosuppression and more careful post-transplant follow-up. Molecular factors, such as HLA and non-HLA antibodies, soluble CD30 molecule (sCD30), Hepatocyte Growth Factor (HGF) and other cytokines, measured before and/or after transplantation in the recipient's blood may be helpful for rejection risk estimation and may also be used as post-transplant rejection onset markers. In our study, we focused on some of the above mentioned factors. We found that ethnicity plays a significant role in the...

Introduction : La dysfonction primaire du greffon (DPG) post-transplantation pulmonaire est la principale cause de décès en phase péri-opératoire. Sa physiopathologie n’est pas encore totalement élucidée mais les lésions d’Ischémie/Reperfusion (I/R) pourraient constituer un facteur important de son développement. L’I/R et la DPG sont caractérisées par des dommages de l’endothélium vasculaire et de l’épithélium alvéolaire, un œdème pulmonaire et une réaction inflammatoire exacerbée. La résorption de l’œdème dépend du rétablissement de l’intégrité fonctionnelle alvéolaire, dont la capacité à réabsorber les ions Na+ (via les canaux ENaC), et secondairement le liquide par les cellules alvéolaires. Nous avons émis l’hypothèse que la dysfonction épithéliale alvéolaire, causée par l’I/R, présente dans les greffons donneurs (GD), jouerait un rôle clef dans le développement de la DPG chez les receveurs. Notre but était d’identifier de biomarqueurs, associés à la dysfonction épithéliale des GD et au développement de DPG chez les receveurs. Méthodes : L’impact d’un protocole mimant une I/R a d’abord été évalué sur des cultures primaires de cellules alvéolaires de rats. Puis, nous avons étudié l’impact de l’I/R in vivo grâce à des modèles de stress inflammatoire par infusion de LPS ou transplantation unilatérale chez le porc. Finalement, des biopsies de tissus de GD ont été recueillies durant les transplantations pulmonaires. Après détermination du grade de DPG chez les receveurs, nous avons étudié les facteurs et les altérations alvéolaires associés. Résultats : Une baisse d’expression des protéines de jonctions serrées (ZO-1), des canaux ioniques ENaC et CFTR ainsi qu’une réduction de la résistance transépithéliale et de la capacité de réparation suite aux lésions ont été observées suite au protocole mimant l’I/R dans le modèle de cultures primaires de cellules alvéolaires. Un traitement avec un activateur du canal K+ KvLQT1 (R L3) a permis d’améliorer la vitesse de réparation, l’intégrité de la barrière épithéliale et l’expression d’ENaC et CFTR. Dans nos modèles animaux, nous avons observé une réponse pro-inflammatoire et une altération des protéines ZO-1, ENaC et CFTR. Nos données préliminaires indiquent aussi une infiltration inflammatoire et une baisse d’ENaC, CFTR et ZO-1, déjà présentes dans les GD ayant subits une I prolongée, chez les receveurs ayant ensuite développés une DPG. Conclusion : Nos résultats soutiennent notre hypothèse du développement d’une dysfonction épithéliale alvéolaire, caractérisée par une altération de biomarqueurs de fonctionnalité et d’intégrité (ENaC, CFTR et ZO-1), en lien avec l’I/R et la DPG.
Background: Primary graft dysfunction (PGD) after lung transplantation is the first cause of death in the perioperative phase. The PGD pathophysiology is not fully elucidated, but Ischemia/Reperfusion (I/R) injury might be an important factor. I/R and PGD both feature endothelial/ epithelial damage, lung edema and inflammation. Edema resorption then depends on the restoration of the alveolar functional integrity, especially the ability of alveolar epithelial cells to reabsorb Na+ (through ENaC channels) and fluid. We hypothesized that alveolar epithelial dysfunction (related to I/R), observed within donor grafts, then plays a key role in the development of PGD in lung recipients. Our goal was to identify novel biomarkers, associated with epithelial dysfunction within donor’s grafts, and then PGD development in recipients. Methods: The impact of a protocol mimicking hypothermic ischemia and reperfusion was first tested on primary rat alveolar epithelial cell cultures. Then, the impact of I/R was studied in vivo using models of inflammatory stress induced by LPS infusion or after unilateral transplantation in pigs. Finally, lung biopsies from donor grafts were collected during lung transplantations. After defining PGD scores within the recipients, associated factors and alveolar alterations were finally analyzed. Results: In primary cell cultures, the protocol mimicking hypothermic I/R induced a decrease in tight junction proteins (ZO-1), transepithelial resistance, wound repair capacity as well as ENaC and CFTR channel expression. Treatment with a KvLQT1 K+ channel activator (R-L3) accelerated the repair rates and enhanced barrier integrity (ZO-1 staining) as well as ENaC and CFTR protein expressions. In the porcine models, an exacerbated inflammatory response was observed along with alveolar damage, lung edema and decreased ZO-1, ENaC and CFTR expressions. Our preliminary data using human samples collected during lung transplantations also indicate an inflammatory response and reduced ENaC, CFTR and ZO-1 expressions, already observed within lung grafts, submitted to longer cold ischemia duration, among lung recipients then developing a PGD. Conclusion: Altogether these data support our hypothesis of an alveolar epithelial dysfunction, featuring an alteration of functionality and barrier integrity biomarkers (ENaC, CFTR and ZO-1), associated with I/R and DPG.

Le rejet chronique se manifeste dans le poumon par la bronchiolite oblitérante (BO), une pathologie inflammatoire et fibrotique menant à l’oblitération des bronchioles. L’étiologie exacte de cette maladie demeure inconnue. Certaines études suggèrent qu'un déséquilibre des leucotriènes (LT) sur les prostaglandines (PG) favorise la fibrose pulmonaire. Les taux des LT et des PG dans le poumon humain post-transplantation sont inconnus. Nous proposons qu'un déséquilibre de cystéinyl leucotriènes (CysLT) sur la PGE2 existe dans le poumon transplanté et pourrait être impliqué dans la pathogenèse de la BO. Aussi, les leucotriènes contribueraient à la fibrose par la transition épithélio-mésenchymateuse (TEM). Afin de vérifier ces hypothèses, nous avons déterminé les taux de CysLT et de PGE2 dans le liquide de lavage broncho-alvéolaire (LBA) provenant de poumons transplantés chez l'homme ainsi que leurs corrélations cliniques. Nous avons également déterminé la capacité des CysLT à induire l’expression des marqueurs de la TEM in vitro. Nous avons découvert des taux de CysLT et PGE2 supérieurs à la normale dans les LBA des greffés. Un pic prédominant de CysLT sur PGE2 est observée à 52 semaines postgreffe et deux facteurs de risque de la BO, les infections au CMV et à l’Aspergillus, sont associés au ratio CysLT/PGE2> 1. In vitro, les CysLT induisent une répression des marqueurs épithéliaux mais n’induisent pas l’expression de marqueurs mésenchymateux chez les cellules épithéliales bronchiolaires.
Chronic rejection occurs, in the lung, in the form of bronchiolitis obliterans (BO), an inflammatory and fibroproliferative disease that leads to the obliteration of the bronchioles. A concept of the pathogenesis of BO has been suggested and several risk factors are associated to it, however, the exact etiology of this disease remains unknown. Studies have suggested that an imbalance of leukotrienes (LT) over prostaglandins (PG) promotes pulmonary fibrosis. The levels of LT and PG in the human lung post-transplantation are unknown. We propose that an imbalance of cysteinyl leukotrienes (CysLT) on PGE2 exists in the transplanted lung and may be implicated in the pathogenesis of BO. We also suggest that leukotrienes contribute to fibrosis through epithelial-mesenchymal transition (EMT). In order to test these hypotheses, we have determined the levels of CysLTs and PGE2 in human transplanted lung bronchoalveolar lavage fluid (BALf) samples and their clinical correlations. We have also determined the capacity of CysLT to induce the expression of EMT markers in vitro. We found high average levels of CysLT and PGE2 in the BAL of transplant patients. A predominant peak of CysLT over PGE2 was observed at 52 weeks post-transplantation and two risk factors for BO, CMV infections and Aspergillus were associated with CysLT/PGE2 ratio> 1. According to our experimental parameters, CysLT can induce the repression of epithelial markers but do not induce the expression of mesenchymal markers in vitro in small airway epithelial cells.

Le polyomavirus BK est un virus très prévalent qui demeure normalement en phase de latence dans l’uroépithélium sans entrainer de complications. Chez les greffés rénaux, il peut cependant se réactiver et mener à une néphropathie pouvant nuire à la survie du greffon. L’immunité du receveur est la pierre angulaire de la prévention et du traitement de cette néphropathie, puisque le seul traitement démontré efficace est une diminution de l’immunosuppression. Cependant, une augmentation non spécifique de l’immunité augmente également le risque de rejet. Notre objectif était donc d’adapter et de valider un protocole transférable en clinique d’immunothérapie adoptive antivirale nous permettant de produire des lignées de lymphocytes T BKvirus spécifiques à partir du sang de patients greffés virémiques, afin de prévenir et traiter ces néphropathies. Nous avons tout d’abord comparé les lignées cellulaires produites à partir de donneurs sains à celles de patients immunosupprimés soumis à une immunosuppression chronique. Par la suite, nous avons adapté le protocole en ajoutant une stimulation à l’aide de cellules dendritiques afin de maximiser l’expansion cellulaire, le statut de différentiation et la spécificité. Bien que les lignées étaient polyclonales, elles n’ont pas démontré de potentiel alloréactif in vivo et in vitro, et ce, malgré une persistance et une prolifération in vivo. Nous avons donc élaboré un protocole qui est prêt à être transféré en étude clinique de phase I/II et qui pourrait nous permettre de prévenir et traiter la néphropathie associée au polyomavirus BK, sans augmenter le risque de rejet.
More than 75% of the population has been exposed to BK polyomavirus and carries latent virus in the uroepithelium without any complications. However, it can reactivates in kidney transplant recipients (KTR) and lead to a nephropathy affecting graft survival. Recipient anti-viral immunity is the cornerstone of BK-virus associated nephropathy prevention and treatment and thus, reduction of immunosuppression is the only well-accepted treatment. Adoptive immunotherapy is a promising solution to this problem, allowing a specific T cell mediated response against this virus without the alloreactive risk. It was demonstrated efficacious for other viral infections in immunocompromised hosts but it has not been used in this specific context. Our objective was to adapt and validate a clinical-compliant protocol to obtain BK-specific T cell lines from viremic KTR and to compare their expansion, differentiation and specificity to ones obtained from healthy donors. Although comparable specificity and differentiation status, cell expansions form KTR were not systematically sufficient for a therapeutic dose. The addition of a stimulation with dendritic cells improved cell expansion in addition to favors a central memory phenotype and refined BKspecificity. Despite polyclonality, T cell lines didn’t demonstrated alloreactivity in a chromium release assay and in vivo. Furthermore, T cell lines could persist and proliferates in vivo. This protocol is ready for a phase I/II clinical trial. This opens the possibility to solve the current conundrum and treat PVAN without increasing rejection risk.

Indiana University-Purdue University Indianapolis (IUPUI)
In the US, more than 1 million burn injuries are reported annually. About 45,000 injuries due to fires and burns result in hospitalization and ten percent of these result in death every year. Advances in burn treatment have led to a reduction in mortality rate over the last decades. Since more patients are surviving the initial resuscitation phase even with very large areas of skin being burned away, wound care has become increasingly important to ensure continued patient survival and improvement. While currently a common treatment for third degree burn wounds, skin grafts have several drawbacks. The availability of donor sites for autografts may be limited, especially in incidences of extensive skin loss. The rejection associated with the use of allografts and xenografts may render them inadequate or undesirable. Even if a suitable graft is found, poor retention due to infection, hematoma, and low vascularity at the recipient site are other drawbacks associated with the use of skin grafts as a primary treatment for severe burn wounds. As such, research has been done into alternative treatments, which include but are not limited to artificial skin, cell therapy, and growth factor application. We propose the delivery of adipose derived stem cells (ASC) in combination with endothelial progenitor cells (EC) via Integra Dermal Regenerative Template (DRT) to promote faster graft vascularization and thus faster healing of wounds. Integra DRT is an acellular skin substitute that consists of a dermal layer composed of bovine collagen and chondroitin-6-sulfate glycosaminoglycan, and an "epidermal" layer, which consists of silicone polymer. This silicone layer is removed after the collagen matrix is adequately vascularized (usually takes 2-3 weeks), and then a thin layer autograft is applied to the top of the neo-dermis. ASC are derived from the stromal-vascular fraction (SVF) of adipose tissue and are a readily available, pluripotent, mesenchymal cell known to promote angiogenesis. They are being explored as a treatment for a myriad of diseases and conditions, including wound healing. In combination with ECs, they form stable microvessel networks in vitro and in vivo. In our work, we found that ASC+EC form stable microvessel networks when cultured on Integra DRT. Also, ASC and ASC+EC conditioned media promoted both survival and migration of human epidermal keratinocytes compared to control medium. In a full thickness wound healing model, using healthy NSG mice, the ASC+EC case showed a significantly higher rate of wound closure compared to control. Based on best linear unbiased estimates (BLUE), the difference between the healing rates of ASC alone treatment and the Control treatment group is -0.45 +/- 0.22 mm²/day (p=0.041), which is not less than 0.025 and thus not statistically significant (Bonferroni Adjusted). However, the BLUE for the difference between the ASC+EC group and the Control group healing rates is -0.55 +/- 0.28 mm²/day (p = 0.017<0.025, Bonferroni Adjusted), which is statistically significant. Histology revealed a significantly higher number of vessels compared to control in both ASC alone and ASC+EC case. CD31 staining revealed the presence of human vessels in ASC+EC treatment scaffolds. We conclude that the combination of ASC and EC can be used to accelerate healing of full-thickness wounds when delivered to site of the wound via Integra. This result is especially compelling due to the fact that the mice used were all healthy. Thus our treatment shows an improvement in healing rate even compared to normal wound healing.