Lymphocytes B mémoire dans la réponse humorale anti- HLA en transplantation d'organe

Les alloanticorps anti-HLA sont dirigés vis-à-vis de différents épitopes des molécules du système HLA. Cette immunisation survient lors d'une transplantation d'organe, de transfusions sanguines ou d'une grossesse. On retrouve aussi ces anticorps, lorsque les techniques de détection sont sensibles, en l'absence de tout évènement immunisant. En transplantation d'organe, rénale en particulier, la présence d anticorps anti-HLA, du fait des lésions de rejet humoral qu'ils induisent, constitue une des premières causes de perte de fonction des greffons à moyen et long terme. Néanmoins, les cellules lymphocytaires qui sont la source de ces anticorps anti-HLA demeurent mal identifiées.Dans la première partie de ce travail, nous avons étudié, dans une cohorte de patients en attente de transplantation rénale, la distribution des différentes sous-populations lymphocytaires B circulantes par cytométrie de flux en relation avec la nature des évènements immunisants vis-à-vis du système HLA, la présence et la diversité des anticorps anti-HLA. Nous avons étudié en parallèle les concentrations sériques de BAFF ("B cell activating factor belonging to the TNF family"), principal facteur impliqué dans la survie et la différenciation des lymphocytes B matures. Nous avons retrouvé une association entre la présence et la diversité des anticorps anti-HLA, et l'augmentation de la proportion de lymphocytes B naïfs activés Bm2, par rapport aux autres sous-populations lymphocytaires B, et indépendamment de l'existence d'évènements immunisants. Les concentrations sériques de BAFF étaient également associées positivement à la présence et à la diversité des anticorps anti-HLA. Ces données suggèrent que l'augmentation des lymphocytes B naïfs activés et des concentrations sériques de BAFF favorise le développement des anticorps anti-HLA à la suite d'un événement immunisant. A l'instar du mécanisme évoqué en auto-immunité, BAFF pourrait intervenir en présence de l'alloantigène en favorisant la survie de clones B alloréactifs.Dans la deuxième partie de notre travail, nous nous sommes intéressés plus particulièrement à l'implication des lymphocytes B mémoire alloréactifs dans la réponse humorale anti-HLA. Pour détecter les lymphocytes B mémoire circulants, nous avons utilisé un test de stimulation polyclonale permettant leur différenciation en plasmablastes puis nous avons recherché et étudié la spécificité des anticorps anti-HLA produits dans les surnageants de culture. Un premier résultat important a été la possibilité de détecter, chez les patients présentant des anticorps anti-HLA, des lymphocytes B mémoire alloréactifs circulants plusieurs années après un événement immunisant. En deuxième lieu, la présence de ces lymphocytes B mémoire était associée au nombre d'évènements immunisants. En effet, les patients ayant développé, en l'absence d'événement immunisant des anticorps anti-HLA - dont nous montrons par ailleurs le caractère potentiellement pathogène - n'ont pas présenté de lymphocytes B mémoire alloréactifs circulants. Enfin, à l'aide du logiciel HLAMatchmaker, nous avons montré que les anticorps produits par les lymphocytes B mémoire étaient dirigés contre un nombre restreint d'épitopes partagés par plusieurs antigènes HLA, ce qui suggère une oligoclonalité du contingent B mémoire alloréactif. Chez les mêmes patients, les anticorps anti-HLA circulants présentaient une diversité de spécificité plus large, étant dirigés contre de multiples épitopes HLA. Ces résultats suggèrent l'existence d'au moins deux types de réponse humorale vis-à-vis des alloantigènes HLA : l'une aboutissant à la production de lymphocytes B mémoire et de plasmocytes à la suite d'une réaction de centre germinatif T-dépendante, l'autre impliquant seulement des plasmocytes, possiblement issus de réponses extra-folliculaires. Les facteurs orientant vers l un ou l autre type de réponse sont encore mal définis mais pourraient impliquer la dose et la voie d'exposition aux alloantigènes.Anti-HLA antibodies are directed against various epitopes of HLA molecules. They develop during organ transplantations, red cell transfusions or pregnancies. But anti-HLA antibodies are also detected with sensitive assays in the absence of any sensitizing event. In renal transplantation, anti-HLA antibodies, through the development of antibody-mediated rejection, represent the first cause of late allograft loss. Nevertheless, the mechanisms and the exact nature of B cells involved in anti-HLA antibodies synthesis are poorly understood.In a first part, we studied by flow cytometry in patients awaiting kidney transplantation the distribution of the different peripheral B cell subsets in relation with immunizing events, titer and diversity of anti-HLA antibodies. We also studied the serum levels of BAFF ("B cell activating factor belonging to the TNF family"), the main factor involved in survival and differentiation of mature B cells. We found an association between the presence and the diversity of anti-HLA antibodies, and the proportion of activated naive Bm2 B cells, at the expense of other subsets, independently of immunizing events. BAFF serum levels were also positively associated with the presence and the diversity of anti-HLA antibodies. These data suggest that the increase in activated naive B cells and in BAFF levels facilitate the development of anti-HLA antibodies, following an immunizing event. Similarly to what is observed in autoimmunity, BAFF could help to the positive selection of alloreactive B cell clones, in the presence of alloantigen.In a second part, we focused on the role of circulating alloreactive memory B cells in anti-HLA humoral response. To detect those alloreactive memory B cells, we used a polyclonal stimulation assay allowing the differentiation of memory B cells into plasmablasts and we studied the specificity of anti-HLA antibodies recovered from culture supernatant. A first important result was the detection, decades after an imunizing event, of specific alloreactive memory B cells, even in the absence of the antigen. The detection of those circulating alloreactive memory B cells was related to the strength of immunizing events, i.e. the number of different immunizing events in the history of patients. Indeed, patients with anti-HLA antibodies with no history of immunizing event had no circulating alloreactive memory B cells. Eventually, with HLAMatchmaker software, we showed that antibodies produced by memory B cells were directed against a limited number of epitopes shared by HLA antigens, which suggests an oligoclonality of the alloreactive memory B cell population. By comparison, serum antibodies displayed a greater diversity, with multiple epitopic specificities. These results suggest two distinct cellular arms of humoral response towards HLA epitopes: medullar plasma cells, involved in long term HLA antibodies synthesis, and memory B cells waiting for a recall response in the presence of the antigen. The factors involved in the choice of those two cellular fates are poorly understood but may involve dose and route of exposition to the alloantigen.PARIS5-Bibliotheque electronique (751069902) / SudocSudocFranceF

Etude de la réponse lymphocytaire T dans l'allergie de l'enfant, au diagnostic et au cours de la désensibilisation

Les maladies allergiques sont de plus en plus fréquentent. Elles atteignent souvent l enfant jeune chez qui l allergie respiratoire et l allergie alimentaire sont les principales pathologies. L unique traitement curatif est l immunothérapie spécifique d antigène (ITA), largement développée dans l allergie respiratoire et encore à ses débuts dans l allergie alimentaire. Pour adapter au mieux la prise en charge du patient, le diagnostic précis de l allergie est indispensable et il n existe actuellement pas d examen biologique totalement fiable. Seul, la présence d IgE spécifiques permet de diagnostiquer une sensibilisation à un allergène mais pas une allergie cliniquement symptomatique. Dans une première partie, nous avons étudié l intérêt d un test fonctionnel, l ELISpot (Enzyme-linked immunosorbent spot), dans le diagnostic de l allergie aux acariens chez l enfant asthmatique. Le nombre de lymphocytes T circulants spécifiques d acariens sécréteur d interleukine (IL)-4 ou d IL-13 était associé à la présence d une allergie symptomatique, indépendamment des IgE spécifiques. Il était plus élevé dans le cas d une rhinite allergique sévère et plus faible dans le cas d une rhinite allergique légère. De plus, il variait au cours de l année en fonction des saisons avec un pic en automne et un pic en début de printemps. Dans une deuxième partie, nous avons étudié l intérêt de l ELISpot dans le diagnostic de l allergie au lait de vache chez l enfant, confirmée par un test de provocation orale en double aveugle. Nous avons décrit que le nombre de lymphocytes T spécifiques de la caséine et sécréteurs d IL-4 et d IL-13 était associé à l allergie au lait de vache avec une sensibilité de 100%. Par ailleurs, le nombre de lymphocytes T spécifiques de la caséine était également associé à la dose maximale de lait tolérée par l enfant.Enfin, dans une troisième partie, nous avons étudié la réponse lymphocytaire T au cours d une ITA sub-linguale (SLIT) d une part et sous-cutanée (SCIT) d autre part, chez des enfants asthmatiques allergiques aux acariens suivis pendant une année. Nous avons décrit une diminution des lymphocytes Th2 (sécréteurs d IL-4 et IL-13) spécifiques d acariens après 12 mois de SLIT associée à une augmentation des cellules sécrétrices d IL-10 (Tr1) spécifiques d acariens après 6 mois de SLIT. De plus, les lymphocytes T régulateurs (CD4+CD25hiCD127loFoxp3+) étaient augmentés après 12 mois de SCIT. Nous n avons pas retrouvé de production accrue d interféron g (IFNg) par les lymphocytes T spécifiques d acariens au cours de la désensibilisation.Au total, ce travail nous a permis de décrire qu un test fonctionnel, l ELISpot, permet de réaliser un diagnostic fiable de l allergie aux acariens et de l allergie au lait de vache chez l enfant. Par ailleurs, l ITA induit une diminution des cellules Th2 et une augmentation des cellules Tr1 par voie sub-linguale ainsi qu une augmentation des Treg Foxp3+ par voie sous-cutanée sans immunodéviation Th2/Th1, chez l enfant allergique aux acariens.Allergic diseases are steadily increasing steadily and especially in children. Allergen specific immunotherapy (desensitization) is the only curative treatment for which accurate diagnosis of allergy is essential. Currently, the presence of specific IgE diagnoses a sensitization to an allergen but not a clinically symptomatic allergy. In a first part, we studied the value of a functional test, the ELISpot (Enzyme-linked immunosorbent spot) in the diagnosis of allergy to house dust mites (HDM). The number of circulating HDM-specific IL-4 and IL-13 secreting T cells was associated with the presence of symptoms, regardless of specific IgE and was higher in severe rhinitis than in mild rhinitis. In addition, it varied according to the season with a peak in autumn and a peak in early spring (wet periods with greater allergen exposure). In a second part, we studied the value of ELISpot for the diagnosis of cow's milk allergy in children, confirmed by double blind placebo control food challenge. We found that the number of casein-specific IL-4 and IL -13 secreting T-cells was associated with allergy to cow's milk. It was also inversely correlated to the cow s milk tolerated cumulative dose. Receiver-operating characteristic (ROC) curve of combined IL-4 and IL-13 analysis was generated. AUC was 0,98 (95% CI 0.90-1.06). For a cut-off of 10 IL-4- and 12 IL-13 secreting T-cells, sensitivity and negative predictive value were 100%.Finally, in the third part, we monitored antigen specific T-cell response in HDM allergic children treated with sublingual ITA (SLIT) on the one hand and subcutaneous ITA (SCIT) on the other hand, during one year. We found a decrease in HDM specific Th2 cells after 12 months of SLIT associated with an increase in HDM specific IL-10 secreting T-cells after 6 months of SLIT. In addition, regulatory T cells (CD4 + CD25hiCD127loFoxp3+) were increased after 12 months of SCIT. In conclusion, this work has allowed us to describe a functional test, the ELISpot, as a reliable tool for the diagnosis of mite allergy and cow's milk allergy in children. In addition, in HDM allergic children, a decrease of Th2 cells and an increase of IL-10 secreting T-cells was found in children treated with SLIT to HDM as well as an increase in Foxp3+ Treg in children treated with SCIT.PARIS5-Bibliotheque electronique (751069902) / SudocSudocFranceF

Preventive and Therapeutic Euphol Treatment Attenuates Experimental Colitis in Mice

BACKGROUND: The tetracyclic triterpene euphol is the main constituent found in the sap of Euphorbia tirucalli. This plant is widely known in Brazilian traditional medicine for its use in the treatment of several kinds of cancer, including leukaemia, prostate and breast cancers. Here, we investigated the effect of euphol on experimental models of colitis and the underlying mechanisms involved in its action. METHODOLOGY/PRINCIPAL FINDINGS: Colitis was induced in mice either with dextran sulfate sodium (DSS) or with 2,4,6-trinitrobenzene sulfonic acid (TNBS), and the effect of euphol (3, 10 and 30 mg/kg) on colonic injury was assessed. Pro-inflammatory mediators and cytokines were measured by immunohistochemistry, enzyme-Linked immunoabsorbent assay (ELISA), real time-polymerase chain reaction (RT-PCR) and flow cytometry. Preventive and therapeutic oral administration of euphol attenuated both DSS- and TNBS-induced acute colitis as observed by a significant reduction of the disease activity index (DAI), histological/microscopic damage score and myeloperoxidase (MPO) activity in colonic tissue. Likewise, euphol treatment also inhibited colon tissue levels and expression of IL-1β, CXCL1/KC, MCP-1, MIP-2, TNF-α and IL-6, while reducing NOS2, VEGF and Ki67 expression in colonic tissue. This action seems to be likely associated with inhibition of activation of nuclear factor-κB (NF-κB). In addition, euphol decreased LPS-induced MCP-1, TNF-α, IL-6 and IFN-γ, but increased IL-10 secretion from bone marrow-derived macrophages in vitro. Of note, euphol, at the same schedule of treatment, markedly inhibited both selectin (P- and E-selectin) and integrin (ICAM-1, VCAM-1 and LFA-1) expression in colonic tissue. CONCLUSIONS/SIGNIFICANCE: Together, these results clearly demonstrated that orally-administered euphol, both preventive or therapeutic treatment were effective in reducing the severity of colitis in two models of chemically-induced mouse colitis and suggest this plant-derived compound might be a potential molecule in the management of inflammatory bowel diseases

A biophysical model of cell adhesion mediated by immunoadhesin drugs and antibodies

A promising direction in drug development is to exploit the ability of natural killer cells to kill antibody-labeled target cells. Monoclonal antibodies and drugs designed to elicit this effect typically bind cell-surface epitopes that are overexpressed on target cells but also present on other cells. Thus it is important to understand adhesion of cells by antibodies and similar molecules. We present an equilibrium model of such adhesion, incorporating heterogeneity in target cell epitope density and epitope immobility. We compare with experiments on the adhesion of Jurkat T cells to bilayers containing the relevant natural killer cell receptor, with adhesion mediated by the drug alefacept. We show that a model in which all target cell epitopes are mobile and available is inconsistent with the data, suggesting that more complex mechanisms are at work. We hypothesize that the immobile epitope fraction may change with cell adhesion, and we find that such a model is more consistent with the data. We also quantitatively describe the parameter space in which binding occurs. Our results point toward mechanisms relating epitope immobility to cell adhesion and offer insight into the activity of an important class of drugs.Comment: 13 pages, 5 figure

Retinal glycoprotein enrichment by concanavalin a enabled identification of novel membrane autoantigen synaptotagmin-1 in equine recurrent uveitis.

Complete knowledge of autoantigen spectra is crucial for understanding pathomechanisms of autoimmune diseases like equine recurrent uveitis (ERU), a spontaneous model for human autoimmune uveitis. While several ERU autoantigens were identified previously, no membrane protein was found so far. As there is a great overlap between glycoproteins and membrane proteins, the aim of this study was to test whether pre-enrichment of retinal glycoproteins by ConA affinity is an effective tool to detect autoantigen candidates among membrane proteins. In 1D Western blots, the glycoprotein preparation allowed detection of IgG reactions to low abundant proteins in sera of ERU patients. Synaptotagmin-1, a Ca2+-sensing protein in synaptic vesicles, was identified as autoantigen candidate from the pre-enriched glycoprotein fraction by mass spectrometry and was validated as a highly prevalent autoantigen by enzyme-linked immunosorbent assay. Analysis of Syt1 expression in retinas of ERU cases showed a downregulation in the majority of ERU affected retinas to 24%. Results pointed to a dysregulation of retinal neurotransmitter release in ERU. Identification of synaptotagmin-1, the first cell membrane associated autoantigen in this spontaneous autoimmune disease, demonstrated that examination of tissue fractions can lead to the discovery of previously undetected novel autoantigens. Further experiments will address its role in ERU pathology

MicroRNA 10a Marks Regulatory T Cells

MicroRNAs (miRNAs) are crucial for regulatory T cell (Treg) stability and function. We report that microRNA-10a (miR-10a) is expressed in Tregs but not in other T cells including individual thymocyte subsets. Expression profiling in inbred mouse strains demonstrated that non-obese diabetic (NOD) mice with a genetic susceptibility for autoimmune diabetes have lower Treg-specific miR-10a expression than C57BL/6J autoimmune resistant mice. Inhibition of miR-10a expression in vitro leads to reduced FoxP3 expression levels and miR-10a expression is lower in unstable “exFoxP3” T cells. Unstable in vitro TGF-ß-induced, iTregs do not express miR-10a unless cultured in the presence of retinoic acid (RA) which has been associated with increased stability of iTreg, suggesting that miR-10a might play a role in stabilizing Treg. However, genetic ablation of miR-10a neither affected the number and phenotype of natural Treg nor the capacity of conventional T cells to induce FoxP3 in response to TGFβ, RA, or a combination of the two. Thus, miR-10a is selectively expressed in Treg but inhibition by antagomiRs or genetic ablation resulted in discordant effects on FoxP3

Value of the First Post-Transplant Biopsy for Predicting Long-Term Cardiac Allograft Vasculopathy (CAV) and Graft Failure in Heart Transplant Patients

BACKGROUND: Cardiac allograft vasculopathy (CAV) is the principal cause of long-term graft failure following heart transplantation. Early identification of patients at risk of CAV is essential to target invasive follow-up procedures more effectively and to establish appropriate therapies. We evaluated the prognostic value of the first heart biopsy (median: 9 days post-transplant) versus all biopsies obtained within the first three months for the prediction of CAV and graft failure due to CAV. METHODS AND FINDINGS: In a prospective cohort study, we developed multivariate regression models evaluating markers of atherothrombosis (fibrin, antithrombin and tissue plasminogen activator [tPA]) and endothelial activation (intercellular adhesion molecule-1) in serial biopsies obtained during the first three months post-transplantation from 172 patients (median follow-up = 6.3 years; min = 0.37 years, max = 16.3 years). Presence of fibrin was the dominant predictor in first-biopsy models (Odds Ratio [OR] for one- and 10-year graft failure due to CAV = 38.70, p = 0.002, 95% CI = 4.00-374.77; and 3.99, p = 0.005, 95% CI = 1.53-10.40) and loss of tPA was predominant in three-month models (OR for one- and 10-year graft failure due to CAV = 1.81, p = 0.025, 95% CI = 1.08-3.03; and 1.31, p = 0.001, 95% CI = 1.12-1.55). First-biopsy and three-month models had similar predictive and discriminative accuracy and were comparable in their capacities to correctly classify patient outcomes, with the exception of 10-year graft failure due to CAV in which the three-month model was more predictive. Both models had particularly high negative predictive values (e.g., First-biopsy vs. three-month models: 99% vs. 100% at 1-year and 96% vs. 95% at 10-years). CONCLUSIONS: Patients with absence of fibrin in the first biopsy and persistence of normal tPA in subsequent biopsies rarely develop CAV or graft failure during the next 10 years and potentially could be monitored less invasively. Presence of early risk markers in the transplanted heart may be secondary to ischemia/reperfusion injury, a potentially modifiable factor