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631	Impact du G-CSF sur le phénotype et les fonctions des cellules NK dans le cadre d’une immunothérapie post-allogreffe de cellules souches hématopoïétiques / Impaired functions and proliferation of NK cells from patient G-CSF mobilized leukapheresis Xiong, Yu 27 July 2016 (has links) Les cellules Natural Killer (NK) sont capables de lyser les cellules tumorales sans la nécessité de reconnaitre un antigène tumoral spécifique. Cette propriété leur confère un avantage par rapport aux lymphocytes T et les rend intéressantes à utiliser en tant que cellules effectrices pour l’immunothérapie adoptive. A ce jour, le potentiel thérapeutique des cellules NK n’a pas été complétement exploré notamment dans le contexte du traitement de la rechute post-allogreffe de cellules souches hématopoïétiques. Actuellement, les patients en rechute post-greffe sont traités avec des injections de lymphocytes du donneur (DLI) parfois issues de petites fractions du greffon de cellules souches hématopoïétiques congelées. Les cellules souches périphériques étant fréquemment utilisées comme source de cellules souches et parfois utilisées comme DLI, nous avons souhaité évaluer l’impact du G-CSF sur le phénotype et les fonctions des cellules NK présentes dans ces fractions. Dans cet objectif, nous avons comparé différentes sources de cellules NK isolées à partir de sang de donneurs sains, de sang mobilisé de donneurs sains ou de patients et observé l’évolution des différentes sous-populations de cellules NK issues de ces prélèvements au décours d’une expansion en présence d’IL-15. Nos résultats ont montré que l’administration de G-CSF diminuait la proportion de cellules NK CD56brightCD16+ au profit d’une population CD16-, diminuait la prolifération des cellules NK lors de l’expansion en culture, et modifiait les propriétés fonctionnelles des cellules NK. / The ability of natural killer (NK) cells to kill tumor cells without the need to recognize a tumor-specific antigen provides advantages over T cells and makes them appealing for a use as effectors for adoptive immunotherapy. However, the full therapeutic potential of NK cell-based immunotherapy has not been fully investigated in the context of leukemic relapse after hematopoietic stem cell transplantation. Today, patients relapsing after hematopoietic stem cell transplantation are often treated with donor lymphocyte infusion (DLI) based on small cell fractions frozen at the time of the stem cell transplantation. Since peripheral blood stem cells are increasingly used as stem cell source and as source of cells for DLI, we aimed to evaluate the impact of G-SCF mobilization on NK cell phenotype and functions. Therefore, we compared the expansion capacity, the phenotype and the function of NK cells from blood for healthy donors, from allogeneic HSCT healthy donors or from autologous HSCT from patients. We also determine the impact of G-CSF on NK cell subset repartition before and after expansion in presence of IL-15. Our results showed that G-CSF administration to patients decreases CD56brightCD16+ NK cell population, proliferation and function. Overcoming this impairment in lymphoid capacity may be important to facilitate post-transplant immunotherapy. Granulocyte-Colony stimulating factor Cellules NK Expansion Cytotoxicité Immunothérapie Granulocyte-Colony stimulating factor Natural killer cells Expansion Cytotoxicity Immunotherapy 616.079 9 571.968
632	Développement d'anticorps bispécifiques pour l'immunothérapie des cancers / Development of bispecific antibodies for cancer immunotherapy Del Bano, Joanie 25 April 2018 (has links) Stimuler la réponse immunitaire anti-tumorale constitue une voie d’avenir indiscutable pour le traitement des cancers. Aujourd'hui, les thérapies ciblées à base d'anticorps ont une place majeure dans l’immunothérapie des cancers du sein de par leur impact positif sur le pronostic des patientes. Cependant, les cancers du sein triple négatifs (TNBC) résistent aux innovations thérapeutiques actuelles, et, par défaut de traitement ciblé efficace, restent de sombre pronostic. Notre équipe développe des stratégies d’immunothérapie à base d'anticorps bispécifiques (bsFabs) conçus à partir de fragments d'anticorps de camélidés qui présentent la particularité de cibler simultanément les cellules immunitaires et tumorales. Ainsi, mon projet visait à évaluer le potentiel anti-tumoral de deux bsFabs sur des modèles précliniques de TNBC à travers leur capacité à activer et à rediriger le système immunitaire contre les cellules tumorales. La finalité du projet est de proposer un nouvel axe de thérapie ciblée susceptible d'améliorer le pronostic des patientes atteintes de TNBC. / Mounting evidence of the key contribution of NK cells in immunity against cancer has boosted the investigations on NK cell-based therapies. Among these strategies, monoclonal antibody-based therapeutics (mAbs) are currently the fastest growing segment of the medicine market. Despite therapeutic innovations, triple negative breast cancers (TNBC) remain insensitive to the current targeted or hormono-therapies. Our objective is to manipulate NK cell functions and tumor targets using an original format of nanobody-based bispecific antibodies (bsFab) to revert the dampened immune response for treating TNBC. Thus, we generate two bsFabs able to crosslink NK and tumor cells. NK antitumor effects driven by mAbs and bsFabs, alone or in combination, were investigated in vitro and in vivo on preclinical TNBC models. Here, we demonstrate the potential of bsFabs to enlarge the number of patients eligible for breast cancer immunotherapy and prompt to consider combination strategies. Anticorps bispécifique Immunothérapie Cellules NK Immuno-Oncologie Cancer du sein triple négatifs Triple negative breast cancer Bispecific antibodies Immunotherapy NK cells Immuno-Oncology
633	L'utilisation de cellules natural killer (NK) comme outil thérapeutique : étude clinique de phase 1 de perfusion de cellules NK du donneur après HSCT : Annexe : Pumilio 2, une protéine de liaison à l'ARN surexprimée dans les cellules NK de patients atteints de LAM, réprime les fonctions des cellules NK / Use of natural killer cells (NK) as a therapeutic tool : phase I clinical study of NK donor lymphocyte infusion after HSCT : Annex : Pumilio 2, a RNA binding protein upregulated in NK cells from AML patients, represses functions of NK cells Taha, Mohammed 18 June 2018 (has links) Les cellules Natural Killer (NK) sont jouent un rôle essentiel dans la surveillance des hémopathies malignes. Cependant, les cellules tumorales développent des mécanismes immunosuppresseurs pour échapper à l'immunité cellulaire NK. Ainsi, le maintien ou l'amélioration des performances des cellules NK sont considérés comme des défis majeurs. Les objectifs de cette partie étaient d'évaluer l'impact de la perfusion de cellules NK activées sur la récupération et la biologie des cellules NK circulantes après l'allo-SCT. Des doses croissantes de cellules NK activées par IL-2 ex-vivo ont été perfusées chez des patients atteints de tumeurs malignes hématologiques 3 mois après allo-SCT. Nos résultats ont montré une fréquence plus élevée des cellules NK dans la périphérie des patients traités. Bien que le phénotype immature soit remarquable peu après le traitement, les cellules NK circulantes, présentaient un état d'activation avec un profil de maturation amélioré après 6 mois de traitement. Nous avons également constaté que l'expression des récepteurs NK activateurs (NKG2D, NKp30 et NKp46) augmentait sur les cellules NK circulantes des patients. De plus, ces cellules ont montré une augmentation significative de la capacité de dégranulation ainsi que de la sécrétion de cytokines (IFN-Ƴ et TNF-α) tout au long de l'étude. Ces différences ont notamment été observées chez les patients ayant reçu des doses plus importantes de cellules NK activées. En conclusion, nous supposons que la perfusion de fortes doses de cellules NK activées ex-vivo pourrait être associée à l'amélioration du phénotype et des fonctions des cellules NK au cours de la reconstitution immunitaire après allo-SCT. / Natural killer (NK) cells are effector lymphocytes of the innate immune system that have the ability to kill transformed cells. They play a critical role in hematological malignancies surveillance, however, tumor cells develop immunosuppressive mechanisms to escape NK cell-mediated killing. So, maintaining or improving NK cell performance is considered a major challenge. Our goals are to evaluate the impact of activated NK cells infusion on the recovery and biology of circulating NK cells post allo-SCT.Three different doses (dose 1: 106 NK cell/Kg, n=3; dose 2: 5x106 NK cell/Kg, n=7; dose 3: >5x106 NK cell/Kg, n=6) of ex-vivo IL-2 activated NK cells were infused into patients with hematological malignancies after all-SCT. Our results showed higher frequency of NK cells in the periphery of patients treated with larger doses of activated NK cells. Although the notable immature phenotype shortly after treatment, the circulating NK cells in patients receiving larger doses of activated NK cells displayed more activation status with improved maturation profile after 6 months of treatment. We also found that the expression of activating NK receptors (NKG2D, NKp30, and NKp46) augmented on circulating CD56dim NK cells of patients receiving larger doses of activated NK cells. Moreover, these cells showed a significant increase in degranulation capacity as well as cytokine secretion (IFN-Ƴ and TNF-α) throughout study period. In conclusion, we hypothesize that infusion of high-dose of ex-vivo activated NK cells could be associated with improvements of NK cell phenotype and function during immune reconstitution after allo-SCT. Cellules NK Immunothérapie Adoptive Pumilio2 Proteine de liaison a l`ARN Leucémie myéloide aigue NK cells Acute myeloid leukemia Adoptive Immunotherapy Pumilio2 RNA-Binding Protein
634	Shiga toxin targeted strategy for chemotherapy and cancer immunotherapy application using copper-free « Click » chemistry Kostova, Vesela 27 November 2015 (has links) Pas de résumé / Recently targeted therapies appeared as attractive alternatives to classical antitumoral treatments. The approach, developed on the concept of targeting drug to cancer cells, aims to spear normal tissues and decrease the side effects. This doctoral dissertation focuses on developing new anticancer targeted treatments in the field of chemotherapy and cancer immunotherapy by exploiting an original targeting moiety, the B subunit of Shiga toxin (STxB). Its specific properties, such as, recognition with its receptor Gb3 overexpressed in cancer cells or in antigen-presenting cells, its unconventional intracellular trafficking, guided the choice of this protein as targeting carrier. This project is based in the use of copper-free Huisgen [3+2] cycloaddition as a coupling method, which led to successful preparation of various conjugates for their respective applications. The concept was first validated by STxB-biotin conjugate. The high yield of the reaction and the compatibility between the targeting carrier and the chemical ligation promoted the design of conjugates for chemotherapy and immunotherapy. Two therapeutical optimizations of previously developed strategy in STxB drug targeting delivery were investigated: synthesis of multivalent drug-conjugates and synthesis of conjugates containing a highly potent anticancer agent. Both approaches exploited three anticancer agents: SN38, Doxorubicin and Monomethyl auristatin F. The disulfide spacer, combined with various self-immolative systems, insured drug release. Two cytotoxic conjugates STxB–doxorubicin (STxB-Doxo) and STxB-monomethyl auristatin F (STxB-MMAF) were obtained in very high yield and demonstrated strong tumor inhibition activity in the nanomolar range on Gb3-positive cells. Based on the results the STxB-MMAF conjugate was investigated on a mouse model. The project aimed also to develop STxB bioconjugates for vaccine applications. Previous studies used B subunit as a targeting carrier coupled to an antigenic protein in order to induce a more potent immune response against cancer. The conjugates were prepared using a commercial linker, requiring modifying the antigen at first place, or by oxime ligation, where slightly acidic conditions promoted the coupling. Thus, the work presented herein proposed an alternative ligation via copper-free click chemistry especially for more sensitive antigenic proteins. Various types of conjugates were synthesised and investigated for their immune stimulation properties. The STxB targeting strategy was also applied to the development of a new vaccine based on coupling the targeting carrier to alpha-GalCer, one of the most potent immune stimulating agents known. The work focused on the synthesis of functionalised alpha-Galcer with an azide handle. Pharmacochimie Cancer Targeting therapy Cancer immunotherapy Shiga toxin Conjugate Ligation Click chemistry Multivalency SN38 Doxorubicin Auristatin Vaccine Ovalbumine Alpha-GalCer 615.19
635	Desenvolvimento e investigação da transferência gênica de p14ARF e interferon-beta em linhagens celulares de melanoma humano / Development and investigation of p14ARF and interferon-beta gene transfer in human melanoma cell lines Mendonça, Samir Andrade 22 November 2018 (has links) O melanoma é um dos tipos de câncer de pele cuja frequência tem crescido nos últimos anos e apresentado elevada taxa de mortalidade, apesar de ter reduzida prevalência. Mesmo havendo um considerável avanço nas propostas terapêuticas nos últimos anos, ainda se vê necessário o desenvolvimento de novas abordagens, sendo a terapia gênica uma promissora possibilidade para tal. Utilizando vetores adenovirais com promotor responsivo à p53 (PGTx beta) para a transferência gênica de p19Arf (proteína supressora de tumor) e interferon-beta (citocina imunomodulatória) em células de melanoma murino com o gene Trp53 selvagem, o nosso grupo demonstrou previamente que a combinação dos dois genes, mas não o tratamento individual, promove efeito citotóxico sinérgico com a liberação de marcadores de morte imunogênica, in vitro; e significativa redução da progressão tumoral acompanhada de uma forte resposta imunológica de linfócitos T CD4+ e CD8+, células NK e neutrófilos contra desafios tumorais, in vivo. Porém, como a translação para modelos de melanomas humanos ainda estava em estágio inicial, ainda não haviam sido confirmamos se esses benefícios também seriam recapitulados. Observações inicias sugeriam que apenas a transferência gênica de interferon-beta seja suficiente para induzir morte celular em linhagens humanas portadoras de TP53 selvagem, sem ainda terem sido identificado o efeito da transferência de p14ARF e nem a necessidade de p53 endógeno para a resposta. Dessa forma, o presente projeto buscou avaliar os efeitos antitumorais provocados pela terapia gênica combinada de p14ARF e interferon-beta em modelos de melanoma humano utilizando linhagens com e sem a via da p53 integra. Para isso, foram utilizadas diferentes linhagens celulares com TP53 selvagem ou com distintas mutações e também foram construídos vetores adenovirais com o promotor constitutivo CMV, tornando assim possível a expressão dos transgenes de maneira independente do status do TP53 endógeno. O presente trabalho revelou que a transferência combinada do interferon-beta e p14ARF revelou vantagem quanto ao estímulo citotóxico e regulação negativa na dinâmica da população em ambas as linhagens UACC-62 e SK-Mel-29, independentemente do estado da via da p53. Na avaliação dos mecanismos de morte foi observado que ambas a linhagens apresentaram marcação positiva para marcadores da via da apoptose, porém com possível participação de outras modalidades de morte-celular, como a necrose, para a linhagem com o TP53 mutado (SK-Mel-29). Além disso, mostramos que os tratamentos potencialmente induzem vias de morte com caráter imunogênico pela secreção de ATP e exposição da calreticulina, sendo este último marcador mais significantemente observado mediante o tratamento combinado. Assim, recapitulamos o benefício observado em modelo murino para a transferência gênica do interferon-beta e p14ARF em modelo de melanoma humano, e investigamos marcadores importantes à translação da proposta terapêutica para o melanoma / Melanoma is one of the types of skin cancer whose frequency has grown in the last years and presents a high mortality rate, despite its low prevalence. Although there has been considerable progress in therapeutic proposals in recent years, it is still necessary to develop new approaches, being gene therapy a promising possibility for this. With the use of adenoviral vectors with a p53 responsive promoter (PGTx beta) for the gene transfer of p19Arf (tumor suppressor protein) and interferon-beta (immunomodulatory cytokine) in murine melanoma cells bearing wild-type Trp53 gene, our group previously demonstrated that the combination of the two genes, but not individual treatment, promotes a synergistic cytotoxic effect with the release of immunogenic death markers in vitro; and significant reduction of tumor progression with a strong immune response mediated by CD4+ and CD8+ T lymphocytes, NK cells and neutrophils in tumor challenges in vivo. However, as the translation for human melanoma models was still at an early stage, it still was not possible to confirm whether these benefits would also be recapitulated in a human model. Initial observations suggested that interferon-beta gene transfer is sufficient to induce cell death in wild-type TP53-bearing human melanoma cell lines, with the effect of p14ARF gene transfer and the role for endogenous p53 in this response yet to be investigated. Thus, the present work aimed to evaluate the antitumor effects induced upon the combined gene transfer of p14ARF and interferon-beta in human melanoma cell lines with and without a functional p53 pathway. For this, different cell lines bearing wild-type TP53 or with different mutations were used and adenoviral vectors with the constitutive CMV promoter were also constructed, making possible the expression of the transgenes independently of the endogenous TP53 status. The present work showed that the combined transfer of interferon-beta and p14ARF was advantageous in cytotoxic stimulation and negative regulation in population dynamics for both cell lines UACC-62 and SK-Mel-29, regardless of p53 pathway status. In the evaluation of the triggered cell death mechanisms it was observed that both cell lines presented positive markers of the apoptosis pathway, but with possible participation of other cell death mechanism, such as necrosis, for the mutated TP53 cell line SK-Mel-29. In addition, we showed that the treatments potentially induced cell death pathways with immunogenic features including the secretion of ATP and calreticulin exposure, being the latter marker more significantly presented after the combined treatment. Thus, we recapitulated the benefit observed in murine model for the gene transfer of interferon-beta and p14ARF in the model of human melanoma, and investigated important markers for the translation of the melanoma therapeutic proposal Cell death Genetic therapy Immunotherapy Imunoterapia Interferon beta Interferon-beta Melanoma Melanoma Morte celular Proteína supressora de tumor p14ARF Terapia genética Tumor supressor protein p14ARF
636	Influência de diferentes concentrações de antígeno na composição de uma vacina anti-HIV baseada em células dendríticas / Effect of diferente amounts of HIV particles on the pulsing MoDCs from HIV infected patients Romani, Nathalia Teixeira 19 October 2018 (has links) Introdução: A infecção pelo HIV causa um profundo comprometimento da resposta imune do hospedeiro, podendo levar à aids. Várias estratégias terapêuticas têm sido testadas ao longo dos anos, entre elas a imunoterapia com células dendríticas diferenciadas a partir de monócitos (MoDCs), pulsadas com HIV-1 inativado. Neste caso, a produção de vírus para o pulso das MoDCs consiste inicialmente no isolamento do vírus a partir de amostras de sangue do paciente e, em seguida, sua expansão em culturas de células CD4. Também deve ser considerado que quantidade excessiva de vírus pode ser tóxica para as MoDCs a serem pulsadas e do mesmo modo, quantidade insuficiente de vírus pode não ser efetiva para ativar uma resposta imune especifica. Neste contexto, a investigação do efeito de diferentes concentrações de vírus sobre o perfil fenotípico e funcional de MoDCs poderia auxiliar na determinação de uma quantidade ótima de vírus para o pulso das MoDCs e contribuir para o aperfeiçoamento da vacina terapêutica. Objetivo: Avaliar o efeito de diferentes quantidades de partículas virais, sobre o perfil fenotípico e funcional das MoDCs. Metodologia: Monócitos obtidos de indivíduos HIV+ foram diferenciados em MoDCs e pulsadas com HIV quimicamente inativado (3 partículas/MoDC, 30 partículas/MoDC, 300 partículas/MoDC). As células foram analisadas com relação ao perfil fenotípico, capacidade de internalizar p24, expressão de CD38, HLA-DR e CD69 e a produção de IFN-y por linfócitos T CD4+ e CD8+ autólogos. Resultados: O pulso com concentrações crescentes de vírus parece não interferir no perfil fenotípico e funcional das MoDCs. Conclusão: As diferentes quantidades de partículas virais utilizadas para o pulso parecem não ser tóxicas para as MoDCs estudadas, não tendo sido observadas diferenças com relação ao perfil fenotípico ou funcional das MoDCs / Introduction: The infection from HIV causes a profound impairment of the host immune response, which can lead to aids. Several therapeutic strategies have been tested over the years, including immunotherapy with monocyte - derived dendritic cells (MoDCs), pulsed with inactivated HIV-1. In this case, the production of virus for the pulse of the MoDCs initially consists of isolating the vírus from the patient\'s blood samples and then it into CD4+ cell cultures. It should also be considered that excessive amount of virus can be toxic to the MoDCs to be pulsed and likewise, insufficiently amount may not be effective for properly activate a specific immune response. In this context, the investigation of the effect of different virus concentrations on the phenotypic and functional profile of MoDCs could assist in the determination of an optimal amount of virus for the pulse of the MoDCs and contribute to the improvement of the therapeutic vaccine. Objectives: To evaluate the effect of different amounts of viral particles on the phenotypic and functional profile of MoDCs. Methods: MoDCs generated from HIV+ individuals were differentiated into MoDCs and pulsed with chemically inactivated HIV (3 particles /MoDC, 30 particles /MoDC, 300 particles /MoDC). Cells were analyzed for phenotypic profile, ability to internalize p24, expression of CD38, HLA-DR and CD69, and the production of IFN-y by autologous CD4 + and CD8 + T lymphocytes. Results: The pulse with increasing concentrations of virus does not seem to interfere in the phenotypic and functional profile of the MoDCs. Conclusion: The different amounts of viral particles used for the pulse appear to be non-toxic to the MoDCs studied, and no differences were observed regarding the phenotypic or functional profile of the MoDCs Antigen presentation Apresentação do antígeno Células dendríticas Cultura de vírus Dendritic cells HIV HIV Immunotherapy Imunoterapia Monocyte-derived dendritic cells Virus culture
637	Immunomodulatory effects and toxicity of mimosa pudica, the sensitive plant. January 1993 (has links) by Cheng Yuk Kwan, Anna. / Thesis (M.Phil.)--Chinese University of Hong Kong, 1993. / Includes bibliographical references (leaves 104-112). / Acknowledgements / Table of Contents --- p.i / Abbreviations --- p.iv / Abstract --- p.vi / List of figures --- p.ix / List of tables --- p.xi / Chapter Chapter One: --- Introduction / Chapter 1.1 --- Objective and scope of the project --- p.1 / Chapter 1.2 --- Literature review of Mimosa pudica / Chapter 1.2.1 --- Morphology of Mimosa pudica --- p.3 / Chapter 1.2.2 --- Chemistry of Mimosa pudica --- p.5 / Chapter 1.2.3 --- Uses in traditional medicine --- p.5 / Chapter 1.2.4 --- Clinical and pharmacological studies of Mimosa pudica --- p.6 / Chapter 1.2.5 --- Toxicology of Mimosa pudica --- p.8 / Chapter 1.2.6 --- Characteristics and toxicology of mimosine --- p.9 / Chapter 1.3 --- Immunomodulation / Chapter 1.3.1 --- Overview of the immune system --- p.11 / Chapter 1.3.2 --- Strategies on the study of immunomodulation of Mimosa pudica --- p.13 / Chapter 1.4 --- Toxicology / Chapter 1.4.1 --- Principles of the toxicological assays / Chapter 1.4.1.1 --- LD50 --- p.17 / Chapter 1.4.1.2 --- Enzyme assays --- p.18 / Chapter 1.4.1.3 --- Subacute toxicity test --- p.24 / Chapter 1.4.1.4 --- Reproductive toxicity test --- p.25 / Chapter Chapter Two: --- Materials and methods / Chapter 2.1 --- Materials / Chapter 2.1.1 --- Mimosa pudica --- p.27 / Chapter 2.1.2 --- Animals --- p.27 / Chapter 2.1.3 --- Chemicals --- p.28 / Chapter 2.2 --- Methods / Chapter 2.2.1 --- Extraction of Mimosa pudica --- p.32 / Chapter 2.2.2 --- Assays for the immunomodulatory effects of Mimosa pudica / Chapter 2.2.2.1 --- Cell preparation / Chapter a) --- Splenocytes --- p.35 / Chapter b) --- Thymocytes --- p.35 / Chapter c) --- Macrophages --- p.36 / Chapter 2.2.2.2 --- Splenocyte proliferation --- p.37 / Chapter 2.2.2.3 --- Thymocyte proliferation --- p.38 / Chapter 2.2.2.4 --- Phagocytic activity of macrophages --- p.39 / Chapter 2.2.2.5 --- Release of IL-1 by macrophages --- p.40 / Chapter 2.2.2.6 --- Plaque forming cells --- p.41 / Chapter 2.2.2.7 --- Restoration on splenocyte blastogenesis of old mice --- p.42 / Chapter 2.2.3 --- Assays for the toxicity of Mimosa pudica / Chapter 2.2.3.1 --- LD50 --- p.43 / Chapter 2.2.3.2 --- Enzyme assays --- p.43 / Chapter 2.2.3.3 --- Subacute toxicity --- p.43 / Chapter 2.2.3.4 --- Reproductive toxicity --- p.44 / Chapter 2.2.4 --- Statistical analysis --- p.44 / Chapter Chapter Three: --- Results / Chapter 3.1 --- Immunomodulatory effects of Mimosa pudica / Chapter 3.1.1 --- In vitro study on the lymphocyte proliferation / Chapter 3.1.1.1 --- Splenocyte proliferation --- p.45 / Chapter 3.1.1.2 --- Thymocyte proliferation --- p.50 / Chapter 3.1.2 --- In vivo study on the lymphocyte proliferation --- p.53 / Chapter 3.1.3 --- Phagocytic activity of macrophages --- p.58 / Chapter 3.1.4 --- Release of IL-1 by macrophages --- p.64 / Chapter 3.1.5 --- Plaque forming cells --- p.67 / Chapter 3.1.6 --- Restoration on splenocyte blastogenesis of old mice --- p.69 / Chapter 3.2 --- Toxicity of Mimosa pudica / Chapter 3.2.1 --- LD50 --- p.72 / Chapter 3.2.2 --- Enzyme assays --- p.75 / Chapter 3.2.3 --- Subacute toxicity --- p.80 / Chapter 3.2.4 --- Reproductive toxicity --- p.85 / Chapter Chapter Four: --- General discussion on the immunomodulatory effects and toxicity of Mimosa pudica / Chapter 4.1 --- Immunomodulatory effects of Mimosa pudica --- p.88 / Chapter 4.2 --- Toxicity of Mimosa pudica --- p.95 / Chapter Chapter Five: --- Concluding remarks --- p.99 / References --- p.104 / Appendix --- p.113 Mimosa Plants, Medicinal Plants, Medicinal--China Drugs, Chinese Herbal--pharmacology Drugs, Chinese Herbal--toxicity Herbal Medicine Herbal Medicine--China Medicine, Chinese Traditional Immunotherapy
638	Implication de l'Oncostatine M dans la genèse et le développement des carcinomes épidermoïdes cutanés / Involvement of oncostatin M in cutaneous squamous cell carcinoma development Simonneau, Marie 21 September 2018 (has links) Le carcinome épidermoïde cutané (CEC) est l'un des cancers les plus fréquents et il est résistant aux traitements chimiothérapeutiques classiques. De nombreuses études montrent que selon leur phénotype les cellules du microenvironnement inflammatoire peuvent inhiber (cellules Th1/M1) ou favoriser (cellules Th2/M2) le développement tumoral. En fonction des cytokines présentes dans ce microenvironnement, il est possible de reprogrammer les cellules immunitaires et de les rendre moins permissives au développement tumoral. L’onconstatine M (OSM) est une cytokine aux effets pléiotropes, elle peut favoriser la prolifération, l’invasion tumorale des cellules tumorales et induire une polarisation immunitaire Th2/M2. Nous avons montré que l'OSM a des effets pro-inflammatoires au niveau cutané et qu’elle module le phénotype des kératinocytes normaux mais son rôle dans les CEC n’est pas décrit. Nous avons donc étudié l’implication de l'OSM dans le développement des CEC. Nous avons montré que l'OSM était surexprimée dans les CEC humains ainsi que d'autres cytokines comme l'IL-6, l'IL-1β, l'IFNγ suggérant une polarisation Th1/M1 des cellules du microenvironnement. In vitro, l'OSM induit l’activation de voies de signalisation pro-tumorales (STAT3 - ERK) au niveau de kératinocytes murins malins ainsi que leur prolifération et leur migration. La greffe de ces cellules chez la souris entraine le développement de CEC associés à une surexpression d'OSM. Enfin, l’absence d'OSM entraine une diminution du volume tumoral de 30% et à une réduction de la polarisation M2. Collectivement, ces résultats suggèrent un rôle pro-tumoral de l'OSM dans le développement des CEC et le blocage de cette cytokine pourrait constituer une nouvelle alternative thérapeutique. / Cutaneous squamous cell carcinoma (cSCC) is one of the most frequent keratinocyte malignancies worldwide and is chemotherapy resistant. Surgery is the curative treatment but there isn’t any alternative in advanced cSCC. Reprogramming tumor microenvironment and tumor immunosuppressive mechanisms is a new therapeutic approach. Indeed, depending on cytokine expressed in tumor microenvironment, immune cells can inhibit (Th1/M1 cells) or enhance (Th2/M2 cells) tumor development. It was previously showed that Onconstatin M (OSM) had pleiotropic effects on cancer cells. OSM can promote cancer by inducing tumor cells motility, invasiveness or by reprogramming immune cells toward a more permissive phenotype (M2 polarization). Our previous data showed that OSM has proinflammatory effects on skin and modulate normal keratinocyte phenotype both in vitro and in vivo. In this study, we hypothesized that OSM could be involved in cSCC development. We showed that OSM was overexpressed in human cSCC as well as other cytokines such as IL-6, IL-1β, IFNγ whereas IL-4 was decreased, suggesting a Th1/M1 polarization of cSCC microenvironment. In vitro, OSM induced STAT-3 and ERK signalization, modified gene expression, promoted proliferation and migration of malignant keratinocyte PDVC57 cells. PDVC57 cells grafted in skin mice led to cSCC development associated to OSM overexpression by immune infiltrated cells. Finally, we showed that the absence of OSM led to a 30% reduction of tumor size and reduced M2 polarization in tumor microenvironment. Collectively, these results support a pro-tumoral role of OSM in cSCC development and suggest a new therapeutic approach targeting this cytokine. Oncostatine M Cytokine Inflammation Microenvironnement tumoral Carcinomes épidermoïdes cutanés Immunothérapie Oncostatin M Cytokines Inflammation Tumor microenvironment Cutaneous squamous cell carcinoma Immunotherapy 616.994 571.978
639	Defining the immune microenvironment in sarcoma : could immunotherapy be part of the treatment strategy in sarcoma patients ? / Etude du microenvironnement immunitaire dans les sarcomes : pourrait-il y avoir une place pour l'immunothérapie dans la stratégie thérapeutique ? Kostine, Marie 20 December 2018 (has links) La chirurgie est la pierre angulaire du traitement curatif des sarcomes, lorsqu’elle est possible. En revanche, en cas de maladie avancée ou métastatique, les traitements systémiques ont une efficacité assez limitée avec un réel besoin de nouvelles options thérapeutiques. Le récent succès de l’immunothérapie dans les tumeurs épithéliales soulève donc la question de la possibilité d’une telle approche dans les sarcomes, et surtout pour quels sous-types histologiques. L’objectif de ce travail de thèse était d’obtenir des données précliniques en caractérisant le microenvironnement immunitaire au sein de trois types de sarcomes potentiellement candidats à l’immunothérapie, prérequis indispensable avant d’envisager une application clinique : 1) Dans le chondrosarcome, l’expression de PD-L1 a été retrouvée exclusivement dans près de 50% des chondrosarcomes dédifférenciés, et s’associait à une infiltration lymphocytaire T et l’expression des molécules HLA de classe I. Ces données incitent donc à inclure les patients avec ce sous type de chondrosarcome dans des essais cliniques évaluant un traitement anti PD-1/PD-L1. 2) Dans l’ostéosarcome, un infiltrat lymphocytaire T était observé de façon bien plus importante dans les lésions métastatiques que dans lésions primitives ou rechutes locales. De plus, l’expression de PD-L1 était retrouvée dans presque 50% des métastases mais pas ou peu dans la tumeur primitive correspondante, traduisant ici une dynamique d’échappement au système immunitaire lors de la progression de la maladie. Une stratégie ciblée sur les lymphocytes T visant à amplifier et potentialiser cette réponse immune préexistante dans les lésions métastatiques pourrait donc offrir un bénéfice clinique. 3) Dans le léiomyosarcome, les molécules HLA de classe I étaient fortement exprimées et l’expression de PD-L1 retrouvée dans 30% des tumeurs de haut grade, également très infiltrées par des macrophages immunosuppresseurs CD163+. Une importante infiltration de macrophages CD163+ était un marqueur indépendant de mauvais pronostic pour la survie, indiquant l’intérêt de d’une approche ciblée visant les macrophages dans ce type de sarcome, éventuellement en association avec un traitement anti PD-1/PD-L1. / Local control with adequate surgery is the cornerstone of sarcoma treatment. However, most sarcoma lack effective systemic therapies in case of advanced disease, emphasizing an unmet medical need for new therapeutic targets. The recent success of immunotherapy in epithelial malignancies raises the question whether such therapies, and which ones, would be applicable in sarcomas. As a prerequisite for therapeutic applications, we characterized the immune microenvironment in three sarcoma subtypes potentially candidate to immunotherapy: 1) In chondrosarcoma, PD-L1 expression was exclusively found in nearly 50% of the dedifferentiated subtype, in association with immune-infiltrating cells and HLA class I expression. These data provide rationale for including such patients in clinical trials with PD-1/PD-L1-targeted therapies. 2) In osteosarcoma, we observed a high density of tumor-infiltrating T cells in metastatic lesions compared to primary tumors and local relapses. Furthermore, PD-L1 positivity in almost half of metastases while mainly negative in the associated primary tumors, emphasises the dynamics of an adaptive mechanism of immune escape. Enhancing the preexisting immune response in metastatic lesions using T-cell-based immunotherapy may offer clinical benefit. 3) In leiomyosarcoma, HLA class I molecules were strongly upregulated and PD-L1 expression found in 30% of high-grade tumors, which were also highly infiltrated with CD163+ immunosuppressive macrophages. CD163+ was found to be an independent poor prognostic factor for overall survival, indicating the need for assessing a macrophage-targeted approach in this tumor type, as single agent or in combination with anti PD-1/PD-L1agents. Sarcome Immunothérapie Pd-1/pd-L1 Hla Macrophages associés aux tumeurs Lymphocytes T Sarcoma Immunotherapy Pd-1/pd-L1 Hla Tumor-Associated macrophages T cells
640	MODULAÇÃO DA RESPOSTA IMUNE FRENTE À INDUÇÃO DE TOLERÂNCIA ORAL A TOXINA DERMONECRÓTICA PRESENTE NO VENENO DE Loxosceles intermedia e TOLERÂNCIA ORAL SOB A PERSPECTIVA DE SISTEMAS COMPLEXOS Delgobo, Murilo 21 February 2014 (has links) Made available in DSpace on 2017-07-21T20:00:01Z (GMT). No. of bitstreams: 1 Murilo Delgobo.pdf: 2288840 bytes, checksum: d9ce3a086e9ee92b92ac76ac76264e04 (MD5) Previous issue date: 2014-02-21 / Brown-Spider’s venom (Loxosceles sp.) is presented as a complex mixture of toxins, able to induce skin necrosis with gravitational spreading, intense inflammatory response, edema induction and increase in vascular permeability in vivo. Recently, the biotechnological potential of the toxins was explored by its use in clinical test, in the study of inflammatory response, as a research tool in cell biology, as a biopesticide and in immunotherapy, through the production of antiserum. In this context, immunotherapy is broadly spread through the production of vaccines, available for the treatment of deleterious reactions developed in accidents. In the present work, we investigated if immunological tolerance induction to dermonecrotic recombinant toxin (LiRecDT1) and its mutated form (LiRecDT1 H12A), through its oral administration, could modulate inflammatory and deleterious responses triggered by dermonecrotic toxin. For this purpose, an oral tolerance protocol was designed, consisting in the administration of 10 μg of LiRecDT1 and LiRecDT1 H12A three times in a week, for three weeks. Adult Swiss mice were further immunized, and oral tolerance induction was observed by reduction in serum levels of IgG antibody anti-toxin when compared with control group. It was observed that mice tolerant to LiRecDT1 H12A present a reduction in paw edema, caused by the injection of 6 μg of dermonecrotic toxin in plantar surface hind paw. Mice tolerized with LiRecDT1 and challenged with 50 μg of dermonecrotic toxin, exhibited higher survival, when compared to control group. This effect was not observed in mice tolerized to LiRecDT1 H12A. The present findings suggested that oral tolerance induction to LiRecDT1 H12A was able to alleviate inflammatory responses triggered by dermonecrotic toxin in paw edema and oral tolerance to LiRecDT1 increase survivability in challenge. The results shown that LiRecDT1 and LiRecDT1 H12A can be explored as a tool in the induction and study of oral tolerance phenomena. The generation of T regulatory cells (Tregs) and following involvement of immunosuppressive cytokines might take part in the modulation of immune response. / O veneno de aranha-marrom (Loxosceles sp.) apresenta-se como uma mistura complexa de toxina, capazes de causar necrose com espalhamento local, intensa resposta inflamatória, indução de edema e aumento da permeabilidade vascular in vivo. Recentemente, o potencial biotecnológico das toxinas foi explorado através de seu uso em análises clínicas, no estudo da resposta inflamatória, como ferramenta de pesquisa na biologia celular, como biopesticidas e na imunoterapia, através da produção de anti-soro. No presente trabalho, foi investigado se a indução de tolerância imunológica à toxina dermonecrótica recombinante (LiRecDT1) e sua forma mutada (LiRecDT1 H12A), através de sua administração oral, poderia modular as respostas inflamatórias e deletérias causadas pela toxina dermonecrótica. Para tal, foi desenvolvido um protocolo para indução de tolerância oral, consistindo na administração de 10 μg de LiRecDT1 e LiRecDT1 H12A três vezes por semana, durante três semanas. Camundongos Swiss fêmeas adultas foram posteriormente imunizadas, e a indução de tolerância foi confirmada pela diminuição nos níveis de anticorpos IgG anti-toxina em relação ao grupo controle, resultado que aponta a obtenção de sucesso na indução de tolerância imunológica. Observou-se que animais tolerantes a LiRecDT1 H12A apresentaram uma diminuição no edema desenvolvida na pata, causado pela aplicação de 6 μg de LiRecDT1 na superfície plantar traseira. Animais tolerizados com LiRecDT1 e desafiados com 50 μg intraperitoneal de toxina dermonecrótica apresentaram maior índice de sobrevivência, quando comparados ao grupo controle. Esse efeito não foi observado em animais tolerizados com LiRecDT1 H12A. Os dados obtidos no presente trabalho sugerem que a indução de tolerância oral à LiRecDT1 H12A é capaz de atenuar o desenvolvimento da resposta inflamatória no edema de pata, enquanto a tolerância oral a LiRecDT1 foi capaz de aumentar a sobrevivência em animais desafiados com LiRecDT1. Os resultados demonstram que as toxinas LiRecDT1 e LiRecDT1 H12A podem ser exploradas como ferramenta na indução e estudo da tolerância oral. A geração de células T regulatórias (Tregs) e subsequente participação de citocinas imunossupressoras devem estar envolvidas na modulação da resposta imune. toxinas biológicas tolerância imunológica imunoterapia venenos de aranha aranha marrom biological toxins immune tolerance immunotherapy spider venoms brown spider

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