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1

Eve, Heather E. "Lenalidomide and the new-generation anti-CD20 antibodies in mantle cell lymphoma". Thesis, Exeter and Plymouth Peninsula Medical School, 2012. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.573119.

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Lenalidomide is a second-generation immunomodulatory drug with clinical activity in mantle cell lymphoma (MCL). In vitro work shows that lenalidomide enhances NK-mediated cytotoxicity against MCL yet the significance of this in vivo remains unproven. Since NK cells are key effectors of antibody-dependent cellular cytotoxicity (ADCC), there is a clear rationale for combining lenalidomide with monoclonal antibodies. However, one concern regarding this is the potential for lenalidomide to downregulate target antigen expression on malignant B Iymphocytes. This thesis presents phase II clinical trial data (EudraCT 2007-005472- 13) confirming the safety, efficacy and immunomodulatory activity of lenalidomide in relapsed/refractory MCL. Using a novel regimen, the benefit of lenalidomide as a low-dose maintenance agent is highlighted. Peripheral T and NK cells increased in responding patients with the NK rise preceded by an initial dip suggesting tumour infiltration. Peripheral Tregs were higher in MCL patients than controls and expanded further following lenalidomide. Bioloqically relevant changes were observed in plasma IL-12p40, IL-7, IL-10, adiponectin and MMP9. A significant correlation between gender and response suggested that female patients were more sensitive to lenalidomide than males. Finally, retrospective analysis of a historical cohort confirmed that thalidomide remains a valid treatment option for MCL patients unsuitable for lenalidomide. The new-generation anti-CD20 antibodies ofatumumab and GA 101 show superiority to rituximab in several B-cell malignancies although data regarding their efficacy in MCL is scarce. Cell culture work using the MCL cell line Granta519 showed ofatumumab was superior to rituximab at inducing complement-dependent cytotoxicity whilst GA 101 was superior to both rituximab and ofatumumab at inducing direct cytotoxicity and ADCC. Combining lenalidomide with these antibodies failed to have any additive cytotoxic effect. Lenalidomide induced significant CD20 downregulation on Granta519 cells. The alternative pan-B cell markers CD19 and, to a lesser extent, CD22 were also downregulated. Thus, if lenalidomide is to be combined with monoclonal antibodies in a clinical setting, sequential administration may be more beneficial than simultaneous administration.
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2

Walshe, Claire Anne. "Signalling cascades induced by type I and II anti-CD20 monoclonal antibodies". Thesis, University of Southampton, 2006. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.436973.

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3

Shan, Daming. "Apoptosis of malignant human B cells by ligation of CD20 with monoclonal antibodies /". Thesis, Connect to this title online; UW restricted, 1998. http://hdl.handle.net/1773/5682.

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DIAS, CARLA R. de B. R. "Estudo comparativo da marcacao do anticorpo anti-CD20 com sup(188)Re". reponame:Repositório Institucional do IPEN, 2010. http://repositorio.ipen.br:8080/xmlui/handle/123456789/9502.

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IPEN/T
Instituto de Pesquisas Energeticas e Nucleares - IPEN-CNEN/SP
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5

Nolan, David Francis Luke. "The synergistic interaction between CD20 monoclonal antibodies and histone deacetylase inhibitors in B cell Non Hodgkin's Lymphoma". Thesis, University of Southampton, 2010. https://eprints.soton.ac.uk/162661/.

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Recent improvements in molecular sub typing of Non Hodgkin’s lymphomas have resulted in targeted therapies becoming incorporated into treatment paradigms. The anti-CD20 monoclonal antibody, Rituximab, has resulted in dramatic improvements in survival for patients with B cell Non Hodgkin’s lymphoma. Histone deacetylase inhibitors are a novel class of anti cancer agents targeting epigenetic regulation. This thesis addresses the interaction between histone deacetylase inhibitors and anti-CD20 monoclonal antibodies, including Rituximab, both in vitro and in vivo. The initial approach identified synergistic induction of apoptosis in a number of B cell lines. In a Ramos xenograft model, combination treatment with suberoylanilide hydroxamic acid (SAHA) and Rituximab reduced tumour growth compared to either agent alone, without discernable toxicity. This effect appears specific to CD20 since monoclonal antibodies directed to other surface molecules (CD32b, CD22, CD37) did not exhibit cooperative effect. Analysis of apoptotic pathways demonstrated that PARP cleavage and caspase processing is significantly higher in cells receiving both treatments. Co-treatment of Ramos cells with the pan caspase inhibitor QVD-OPH abolished the synergy observed with CD20 monoclonal antibodies, suggesting that caspase processing is necessary for synergy. Treatment of Ramos cells stably transfected to overexpress Bcl-2 resulted in loss of synergy with Rituximab, but not with the type II CD20 mAb B1 (Tositumomab). Gene expression array analysis of Ramos cells was performed. Geneset enrichment analysis identified significant regulation of NFқB target genes in some genesets (Rituximab Vs control, p<0.001) with a number associated with apoptosis and B cell activation (Bcl2A1, LTA, CD69) which were confirmed using RT-Q-PCR. This novel combination elicits the induction of apoptosis in vitro, potentially through regulation of Bcl-2 family proteins and should be tested in a phase I/II clinical trial.
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6

Reslan, Lina. "Comparison of the cytotoxic mechanisms of anti-CD20 monoclonal antibodies Rituximab and GA101 in Chronic Lymphocytic Leukemia". Thesis, Lyon 1, 2010. http://www.theses.fr/2010LYO10346/document.

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CD20 est une cible thérapeutique validée pour l’immunothérapie des néoplasmes lymphoïdesdes cellules B, incluant la Leucémie Lymphoïde Chronique (LLC). Nous avons comparé les effets de rituximab et de GA101 (nouvel anticorps anti-CD20) contre les cellules LLC fraiches in vitro. Le marquage avec Annexine V a démontré une induction de l’apoptose après l’exposition au rituximab et GA101.Contrairement au rituximab, GA101 induisait une réduction du potentiel transmembranaire mitochondrial, uneffet qui peut être partiellement inhibé par la cyclosporine A et qui est partiellement caspase-dépendant. GA101induisait aussi la production des espèces d’oxygènes réactives. L’analyse du niveau d’expression des protéinespro- et anti-apoptotiques après exposition aux anticorps a démontré une forte hétérogénéité entre les échantillons.Bax subissait une activation de conformation et une translocation mitochondriale suite à l’exposition aux anticorps d’une manière caspase-indépendante. GA101, mais pas rituximab, induisait le clivage des caspase-8, -9et -3. En transfectant les cellules LLC avec un siRNA ciblant Bcl-xL utilisant la sonoporation, nous avons trouvéque la réduction du niveau d’expression de Bcl-xL est associée à une augmentation de la sensibilité aux anticorps. Nos résultats suggèrent que les voies de signalisation apoptotiques diffèrent entre rituximab et GA101avec une implication de la voie mitochondriale avec le GA101. L’inhibition de Bcl-xL peut constituer une façon pour sensibiliser les cellules LLC aux effets apoptotiques des anticorps anti-CD20
CD20 is a validated target for the immunotherapy of B lymphoid neoplasms, including ChronicLymphocytic Leukemia (CLL). We compared the activities of rituximab and GA101 (novel anti-CD20 antibody)on fresh human CLL cells in vitro. AnnexinV staining demonstrated induction of apoptosis after exposure torituximab or GA101. Unlike rituximab, GA101 induced a reduction of the mitochondrial transmembranepotential, an effect which could be partially inhibited by cyclosporin A and which was partially caspasedependent.GA101 was also found to induce the production of Reactive Oxygen Species. Analysis of pro- andanti-apoptotic protein content after exposure to antibodies demonstrated a strong degree of heterogeneity between samples. Bax underwent conformational activation and mitochondrial translocation upon exposure toantibodies in a caspase-independent manner. GA101 but not rituximab induced cleavage of caspase-8, -9 and -3.By transfecting CLL cells with anti-Bcl-xL siRNA using a sonoporation method, we found that reduction of BclxLcontent was associated with increased sensitivity to these antibodies. Our results suggest that apoptoticsignalization pathways differ between rituximab and GA101 with a greater involvement of the mitochondrialpathway for GA101. Inhibition of Bcl-xL could constitute an approach to sensitize CLL cells to the apoptoticeffects of anti-CD20 antibodies
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7

Spasevska, Ivana. "The role of EGR-1 and calcium influx in the antitumor activity of anti-CD20 monoclonal antibodies". Thesis, Lyon, 2017. http://www.theses.fr/2017LYSE1304/document.

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Les anticorps monoclonaux (AcM) anti-CD20 sont essentiels pour le traitement du lymphome non hodgkinien et de la leucémie lymphoïde chronique (LLC). Les AcM agissent soit en activant directement la signalisation apoptotique dans les cellules cibles, soit via le système immunitaire. Dans une étude préclinique, nous avons montré que le traitement avec AcM anti-CD20, rituximab et GA101, induit l'expression de la protéine early growth response 1 (EGR-1) (Dalle et al., 2011). EGR-1 est un facteur de transcription régulé par le calcium (Ca2+) et CD20 est impliqué dans la régulation du flux calcique transmembranaire. Nous avons donc étudié le rôle d'EGR-1 et du flux Ca2+ dans l'activité cytotoxique des AcM anti-CD20. Nous avons montré qu'EGR-1 est rapidement induit suite à l'exposition au rituximab et à GA101. La baisse de l'expression d'EGR-1 par shRNA a supprimé l'effet cytotoxique du GA101 à la fois in vitro et in vivo, indiquant qu'EGR-1 est requis pour la mort cellulaire médiée par CD20. De plus, la surexpression d'EGR-1 augmente la sensibilité au GA101 in vitro et in vivo. En outre, nos résultats indiquent que les AcM anti-CD20 induisent un flux Ca2+. Le blocage du flux Ca2+ par inhibiteurs de canaux calciques (ICC) a aboli l'induction d'EGR-1 ainsi que l'efficacité du GA101 in vivo et ex vivo dans des échantillons de LLC. Plus important, nos données indiquent que les patients recevant des ICC ont une moins bonne réponse au traitement par les AcM anti-CD20. En conclusion, nous avons identifié EGR-1 comme potentiel biomarqueur pour prédire la réponse à la thérapie anti-CD20 et démontré que les ICC ont un impact négatif sur l'efficacité des AcM anti-CD20 chez les patients
Anti-CD20 monoclonal antibodies (mAbs) are an essential component of the treatment of patients with non-Hodgkin's lymphoma and chronic lymphocytic leukemia (CLL). They mediate their antitumor effects by activating the immune system or by direct apoptotic signaling in target cells. In a previous preclinical study, we showed that treatment with anti-CD20 mAbs, rituximab and GA101, resulted in upregulated expression of early growth factor 1 (EGR-1) (Dalle et al. 2011). EGR-1 is a calcium (Ca2+) regulated transcription factor and CD20 is hypothesized to regulate transmembrane Ca2+ flux. Therefore, we aimed to assess the role of EGR-1 and Ca2+ flux in the cytotoxic activity of anti-CD20 mAbs. We have shown that EGR-1 expression is rapidly upregulated in CD20+ cells following rituximab and GA101 exposure. Decreasing EGR-1 expression by shRNA abolishes the direct cytotoxic effect of GA101 both in vitro and in vivo, indicating that EGR-1 is required for CD20-mediated cell death. Additionally, the overexpression of EGR-1 enhances the cytotoxic activity of GA101 both in vitro and in vivo. Furthermore, our results indicate that anti-CD20 mAbs induce calcium influx. Blocking the Ca2+ flux with calcium channel blockers (CCB) abolishes EGR-1 induction and impaires the GA101 efficacy in vivo and ex vivo in CLL blood samples. More importantly, our data indicate that patients receiving CCBs and anti-CD20 therapy have worst progression free survival and overall survival. In conclusion we have identified EGR-1 as a potential biomarker to predict response to anti-CD20 therapy. We demonstrated that co-treatement with CCBs negatively impacts the outcome of patients receiving anti-CD20 mAbs
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8

AKANJI, AKINKUNMI G. "Estudo de marcação com iodo-131 de anticorpo monoclonal anti-CD20 usado na terapia de linfoma nao-hodgkin". reponame:Repositório Institucional do IPEN, 2006. http://repositorio.ipen.br:8080/xmlui/handle/123456789/11488.

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IPEN/D
Instituto de Pesquisas Energeticas e Nucleares - IPEN/CNEN-SP
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9

Nishida, Michio. "Novel humanized anti-CD20 monoclonal antibodies with unique germline VH and VL gene recruitment and potent effector functions". Kyoto University, 2008. http://hdl.handle.net/2433/124332.

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10

AKANJI, AKINKUNMI G. "Estudo de conjugação do anticorpo anti-CD20 para marcação com radionuclídeos metálicos ou lantanídeos". reponame:Repositório Institucional do IPEN, 2013. http://repositorio.ipen.br:8080/xmlui/handle/123456789/28021.

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Linfomas são cânceres que se iniciam a partir da transformação maligna de um linfócito no sistema linfático. Os linfomas são divididos em duas categorias principais: os linfomas de Hodgkin e todos os outros linfomas, denominados linfomas não-Hodgkin (LNH). Os pacientes com LNH são comumente tratados com radioterapia apenas ou combinada com quimioterapia utilizando-se de anticorpo monoclonal anti-CD20, principalmente o rituximab (MabThera®). O uso de anticorpos monoclonais (Acm) conjugados à quelantes bifuncionais radiomarcados com radionuclídeos metálicos ou lantanídeos é uma realidade de tratamento para portadores de LNH pelo princípio de radioimunoterapia (RIT). Este estudo concentrou-se nas condições de conjugação do anticorpo monoclonal rituximab (MabThera®) com grupamentos quelantes bifuncionais DOTA e DTPA. Na marcação dos Acm conjugados com lutécio-177, foram estudadas as condições de pré-purificação do Acm, condições de conjugação, determinação de número de quelantes acoplados à molécula do anticorpo, purificação do anticorpo conjugado, radiomarcação do anticorpo conjugado, com lutécio-177, purificação do anticorpo marcado, a ligação específica in vitro dos compostos marcados às células Raji, e distribuição biológica em camundongos BALB/c sadios. As três metodologias empregadas na pré-purificação do anticorpo (diálise, cromatografia de exclusão molecular com coluna Sephadex G-50 e ultrafiltração) demonstram-se eficientes e proporcionaram recuperação da amostra superior a 90%. A metodologia de ultrafiltração foi considerada a mais simples e prática, podendo ser aplicada a procedimentos rotineiros de produção de radiofármacos. Além disso, proporcionou a recuperação final de amostra de 97% em microlitros. Nas conjugações do anticorpo com os quelantes DOTA e DTPA em razões molares diferentes do Acm:quelante, observou-se número de grupamentos quelantes acoplados à molécula do Acm proporcional à razão molar estudada. Quando foi avaliada a influência de condições diferentes de conjugação no número de quelantes acoplados à molécula do Acm, não foram observadas diferenças significativas, com resultados de pureza radioquímica (PR) inferior a 80% em todas as condições estudadas. Na comparação de métodos de purificação do Acm conjugado, a abordagem inédita apresentada neste estudo, na qual a cromatografia de exclusão molecular foi combinada com a ultrafiltração resultou em maior eficiência na purificação e preservação da estrutura do anticorpo. Nos estudos de radiomarcação do anticorpo conjugado com DOTA e DTPA, os imunoconjugados de DTPA apresentaram, de forma geral, maior eficiência de marcação com resultados reprodutíveis quando comparados com os imunoconjugados de DOTA, considerando-se as diferentes razões molares utilizadas. As metodologias cromatográficas empregadas no controle de pureza radioquímica do composto radiomarcado proporcionaram a discriminação das diferentes espécies radioquímicas no meio de marcação. A metodologia de purificação do composto conjugado e radiomarcado utilizada proporcionou a obtenção de compostos com alta pureza radioquímica, 97,4±1,3% (DOTA 1:50) e 98,7±0,2% (DTPA 1:50). Nos estudos de ligação específica às células tumorais Raji, o anticorpo conjugado com quelante DTPA nas razões molares de 1:50 e 1:20 apresentaram perfil semelhante de ligação, com aumento da porcentagem de ligação específica proporcional à concentração celular, enquanto que o imunoconjugado na razão molar de 1:10 apresentou alta porcentagem de ligação não específica. Os resultados obtidos nos estudos de biodistribuição in vivo do anticorpo conjugado e radiomarcado nem sempre se mostraram compatíveis com a biodistribuição de anticorpos radiomarcados íntegros. No caso do quelante DOTA, o imunoconjugado obtido a partir da razão molar 1:20, apresentou melhores características de biodistribuição. No caso do quelante DTPA, a razão molar utilizada pareceu refletir diretamente no clareamento sanguíneo do anticorpo e todas as razões molares utilizadas apresentaram instabilidade in vivo.
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IPEN/T
Instituto de Pesquisas Energéticas e Nucleares - IPEN-CNEN/SP
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11

Marques, Carlos Humberto. "Aspectos fundamentais à implantação da tecnologia de produção de anticorpos monoclonais humanizados com potencial aplicação terapêutica". Instituto de Tecnologia em Imunobiológicos, 2005. https://www.arca.fiocruz.br/handle/icict/5781.

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Fundação Oswaldo Cruz. Instituto de Tecnologia em Imunobiológicos. Rio de Janeiro, RJ, Brasil / Fundação Oswaldo Cruz. Instituto Oswaldo Cruz. Rio de Janeiro, RJ, Brasil.
Os anticorpos monoclonais possuem diversasaplicações em transplantes, na composição de conjuntosde reativos para diagnóstico, grande variedade de doenças auto-imunes e, principalmente, na terapia do câncer. A tecnologia de produção de anticorpos monoclonais recombinantes revolucionou a geração de imunoglobulinas, possibilitando a obtenção de anticorpos humanizados dirigidos a uma grande variedade de antígenos específicos. A baixa seletividade das metodologias atuais para diagnóstico e terapia de neoplasiasconstitui um dos principais empecilhospara a prática oncológica. Nesse particular, a utilização de imunoglobulinas submetidas à engenharia genética já é uma realidade e significa um avanço estratégico, abrangendo cerca de 25% do mercado biofarmacêutico global de proteínas terapêuticas. Este trabalho aponta os aspectos fundamentais à concretização da metodologia de humanização de anticorpos por transplante das regiões determinantes de complementaridade – CDR, com ênfase em uma proposta de produção do anticorpo anti – CD20 contrao Linfoma Não-Hodgkin. A introdução do Instituto de Tecnologia emImunobiológicos - Bio-Manguinhos nesse promissor e importante mercado de biofármacos através da implantação da metodologia de humanização do anticorpo monoclonal murino anti-CD20 é objeto desta dissertação. Viabilizar sua produção torna-se extremamente importante, tanto para a identificação precisa e precoce da enfermidade, quanto para atender um segmento do mercado brasileiro ainda desprovido de tratamento abrangente e eficaz. A apresentação do estudo dos anticorpos, sua estrutura e características, o estudo dosdiferentes sistemas de expressão, cultivo, purificação,bem como a proposta de reestruturação e redimensionamento do Laboratório de Tecnologia de Anticorpos Monoclonais, parcerias, colaborações, recursos humanos necessários e aspectos de mercado, são aqui considerados.
Monoclonal antibodies (Mabs) have several applications in transplants, reagents for diagnosis, a great variety ofauto-immune diseases and mainly, in cancer therapy. Mabs production employing recombinant echnologymade a revolution in immunoglobulinsgeneration, enabling the production of humanized antibodiesthat recognize specific antigens. The low selectivity of the current techniquesfor neoplasm diagnosis and therapy is one of the major impediments for oncology practice. In this regard, the use of eneticallyengineered immunoglobulins has become a reality and meansa strategic development comprising around 25% of the global biopharmaceutical market. This work shows the most important aspects in Mabs humanization through complementary determining regions (CDR) graft methodology, emphasizing a proposal ofanti-CD20 Mab production against non-Hodgkin lymphoma. Introducing the Instituto de Tecnologia emImunobiológicos – Bio-Manguinhos in this important and promising biopharmaceutical market through the establishment of humanization methodology is the main object of this dissertation. Making humanized Mabs production feasible is veryimportant not only for the earlyand precise identification of illnesses, but also to meet a demand of the Brazilian market that still lacks comprehensive and efficient treatment. The study of Mabs, their structureand properties, expression systems, cultivation, purification, new dimensions and structure of the laboratory, partnerships, cooperation,human resources and market analysis are considered herein.
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12

Carpio, Virna Nowotny. "Associação entre a fração do complemento C4d, anticorpos anti-hla doador específicos e infiltrados de células B em enxertos renais com rejeição". reponame:Biblioteca Digital de Teses e Dissertações da UFRGS, 2012. http://hdl.handle.net/10183/139415.

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Introdução: O fragmento C4d e os anticorpos anti-HLA doador específicos (DSA) são marcadores de resposta humoral em enxertos renais com rejeição, mas o papel das células B nesse processo ainda não é claro. Neste estudo foi avaliada a correlação entre C4d, DSA e células B de enxertos com disfunção e sua associação com aspectos morfológicos, função e sobrevida do rim transplantado. Material e Métodos: A marcação para C4d, células B CD20+ e plasmócitos CD138+ foi realizada por imunoperoxidase em biópsias por indicação de 110 receptores de transplante renal. Positividade para CD20 e CD138 foi definida por curva ROC (≥5 céls./mm2). O soro coletado concomitante a biópsia foi testado para DSA classe I e classe II. Estes marcadores foram correlacionados com dados clínicos e do transplante, a histopatologia de Banff e a evolução do rim transplantado. Resultados: Depósitos de C4d e DSA circulantes foram detectados em 100% e 70% dos pacientes com rejeição mediada por anticorpos (RMA) respectivamente, e nos casos de rejeição aguda celular (RAC) em 42% (p<0,001, vs. RMA) e 28% (p=0,003, vs. RMA). Estes dois marcadores correlacionaram-se positivamente (r=0,31, p=0,016). Houve correlação significativa entre DSA e plasmócitos CD138+ (r=0.32 p=0,006), mas as células CD20 e CD138 não se correlacionaram entre si. As células CD138+ predominaram na RMA, associadas com maior painel pré-transplante e DSA, mas não a C4d, e as células CD20+ predominaram na RAC e nas biópsias com fibrose intersticial/atrofia tubular, associadas a maior incompatibilidade HLA e a retransplantes. Pacientes com C4d+ tiveram pior função e sobrevida do enxerto em três anos de transplante, e aqueles com DSA+ uma pior 7 sobrevida do enxerto. Positividade para CD20 ou CD138 não foi preditiva da função ou sobrevida do enxerto. Na análise multivariada, somente o C4d foi fator de risco para perda do enxerto. Conclusões: Esses resultados confirmam o valor prognóstico do C4d e dos DSA para uma pior evolução do enxerto renal, e sugerem uma associação das células B CD20+ com parâmetros de rejeição celular e dos plasmócitos CD138+ com marcadores de resposta humoral. Entretanto, nesse estudo o infiltrado de células B na biópsia do enxerto não foi preditivo de uma pior evolução do rim transplantado.
Introduction: The fragment C4d and the donor specific anti-HLA antibodies (DSA) are markers of the humoral response in rejecting kidney grafts, but the role of B cells in this process is still unclear. In this study we evaluated the correlation between C4d, DSA and B cells in dysfunctional grafts, and their association with morphological features, and graft function and survival. Material and Methods: The staining for C4d, CD20+ B cells and CD138+ plasmocytes were done by immunoperoxidase in 110 kidney graft biopsies for cause. Positivity for CD20 and CD138 were established by ROC curve (≥5 cells/mm2). Serum collected at biopsy were tested for anti-HLA class I and II antibodies. These markers were correlated with clinical and transplant characteristics, Banff histopathology and graft outcomes. Results: C4d deposits and circulating DSA were detected in 100% and 70% of the patients with antibody-mediated rejection (AMR) respectively, and in cases with acute cellular rejection (ACR) in 42% (p<0.001, vs. AMR) and 28% (p=0.003, vs. AMR), respectively. Both markers were positively correlated (r=0.31, p=0.016), and there was also a significant correlation between DSA and plasmocytes CD138+ (r=0.32 p=0.006). CD20 and C138 cells were not siginificantly correlated. Plasmocytes CD138+ predominated in AMR, and were associated with higher pre transplant PRA and DSA positivity, but not with C4d. CD20+ B cells were highly expressed in ACR and in biopsies with interstitial fibrosis and tubular atrophy, in association with more HLA mismatches and re-transplants. Patients with C4d had poorer graft function and survival, and those 9 with DSA + also had a worse graft survival in three years of transplant. CD20 or CD138 cells were not predictive of graft outcomes. In multivariated analysis, only C4d remained a risk factor for graft loss. Conclusion: These results confirm the prognostic value of C4d and circulating DSA for a worse kidney graft outcome, and suggest an association of CD20+ B cells with parameters of cellular rejection whereas CD138+ plasmocytes correlated with markers of the humoral response. However, in this study the B cell infiltrate in graft biopsy was not predictive of adverse outcomes to the transplanted kidney.
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Harvey, Melanie Louise. "CD40 antibodies for the treatment of human malignancy". Thesis, University of Southampton, 2002. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.274432.

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CD40 is an important antigen involved in immune regulation and anti-CD40 antibody therapies against human CD40 expressing tumours may be particularly advantageous. The antibody could induce tumour response in two ways. Firstly it might have a direct anti-tumour effect and secondly it could 'boost' the immune system to provide a heightened immune response that evades tumour tolerance. This project has explored the effects of CD40 ligation of a variety of CD40 expressing tumours including transformed human B cell lines (RL and Daudi), human epithelial cell lines (MG79 [ovarian] and Caski [cervical]) and primary human B cell non-Hodgkin's lymphomas obtained, with consent, from patients undergoing excision lymph node biopsy or splenectomy. The ligation of CD40, on transformed human B cell lines, using chinese hamster ovary cells transfected to express human CD40L and human soluble CD40L has shown significant cellular growth inhibition (p
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14

Ilkow, Veronica Franciszka. "Engineering IgE antibodies and CD23 for therapeutic discovery". Thesis, King's College London (University of London), 2018. https://kclpure.kcl.ac.uk/portal/en/theses/engineering-ige-antibodies-and-cd23-for-therapeutic-discovery(54f73d64-5c16-42c4-9dea-42855873eeb6).html.

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Immunoglobulin E (IgE) is fundamental to the allergic response and the functions of IgE are mediated by its Fc region binding to two receptors, FcεRI and CD23 (FcεRII). The interaction of IgE with other proteins have complicated our investigations of the unique role each receptor plays. To solve this, a small-scale library of IgE-Fc proteins was designed with two key positions, one at each receptor-binding site mutated. The unpredictable allosteric nature of IgE prevents rational engineering approaches, thus the design of a membrane-bound IgE-Fc-GFP-tagged protein allowed for the generation of a membrane-surface display library of stable cell lines. A FACS selection assay identified IgE-Fc proteins with weakened binding to a single IgE-receptor, which serves as a proof-of-principle for this concept. Additional studies into human CD23 and the differences between it and murine CD23 revealed additional levels of regulation for IgE-binding not seen in other species and this is due to its unique properties. Human CD23 is an unusual antibody receptor, being a calcium dependent (C-type) lectin that has lost its carbohydrate binding capability. Ca2+ binds to and increases CD23’s affinity for IgE, and one of two Ca2+ binding sites usually present in C-type lectins is absent in human but present in murine CD23. To understand if the loss of the second Ca2+ binding site has led to a regulatory gain/loss of function in human CD23, a panel of CD23 mutant proteins with increasingly ‘mouse-like’ sequences was generated. The insertion of the second Ca2+ binding site was verified by HSQC-NMR whilst molecular dynamic simulations provided a means of understanding the flexibility of the proteins. It revealed that binding of two Ca2+ ions tethers the soluble CD23 loops into position in the most mouse-like mutant protein, limiting possible conformations for IgE binding. Complementary Biacore experiments indicated that higher calcium binding affinity may have come at a cost of weakened IgE binding, as data in the presence and absence of Ca2+ showed decreased binding affinities of the proteins for human IgE. This regulatory difference between murine and human soluble CD23 could inform the development of CD23/IgE inhibitor therapeutics for the treatment of allergy.
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15

Bensalem, Amina. "Pharmacocinétique et relation dose-concentration-effet du rituximab dans la polyartrite rhumatoïde et les vascularités associées aux anticorps anti-cytoplasme des neutrophiles". Thesis, Tours, 2019. http://www.theses.fr/2019TOUR3302.

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Le rituximab est un anticorps monoclonal (AcMo) IgG1 chimérique qui cible le CD20, une protéine présente à la surface de la plupart des lymphocytes B. Il est indiqué dans la polyarthrite rhumatoïde (PR) et est utilisé dans les vascularites associées aux anticorps (ANCA) anti-cytoplasme des neutrophiles (AAV). Il existe une grande variabilité interindividuelle de la pharmacocinétique (PK) du rituximab et de sa relation concentration-réponse. Le rituximab se lie au CD20, et les complexes rituximab-CD20 formés sont éliminés par le système immunitaire. L’élimination médiée par la cible n'a jamais été décrite dans les maladies inflammatoires auto-immunes. Ce travail de thèse visait à étudier la PK et la relation concentration-réponse du rituximab par modélisation PK et pharmacocinétique-pharmacodynamique (PK-PD) de population. Ces travaux ont été réalisés grâce à : - 52 patients atteints de PR, suivis dans le Service de rhumatologie du CHRU de Tours, où les concentrations de rituximab, la numération CD4+ et le score d'activité de la maladie sur 28 articulations (DAS28) ont été mesurés. - 92 patients de l'essai RAVE, où les concentrations de rituximab, d'anticorps anti-protéinase 3 (PR3-ANCA) et d’anti-myéloperoxydase (MPO-ANCA) ont été mesurées. Chez les patients atteints de PR, la PK du rituximab a été décrite à l'aide d'un modèle à bicompartimental. Aucune élimination médiée par la cible n'a été détectée. Cela peut être dû à (i) une faible quantité d'antigène-cible par rapport à l’oncologie, et/ou (ii) à des données de PK peu denses. Chez les patients atteints d’AAV, une élimination non-linéaire médiée par la cible a été détectée au début du suivi. Un modèle TMDD simplifié a été utilisé, où le rituximab se fixait de façon irréversible sur le CD20, modélisé en tant que variable «latente». La variable latente peut être en partie interprétée comme la fraction de CD20 (circulante ou exprimée sur la membrane des cellules B) et disponible pour la liaison au rituximab. L'élimination médiée par la cible, négligeable, à la fin du suivi dans les AAV, peut être due aux numérations de cellules B faibles à la fin du suivi. La relation quantitative entre la déplétion des cellules B du sang, des cellules immunitaires, et la réponse clinique reste floue, aussi bien dans la PR que dans les AAV. De plus, cette relation, très variable selon les patients, n’a jamais été quantifiée à l’aide de la modélisation PK-PD. - Dans la PR, les relations entre les concentrations de rituximab et les numérations CD19+, entre les numérations CD19+ et CD4+, et entre les numérations CD4+ et le DAS28 ont respectivement été décrites à l'aide de modèles de durée de vie cellulaire « cell lifespan », de réponse indirecte et directs (Emax). Cette étude a montré que (i) l’amplitude de la déplétion CD19+ n’était pas associée à une déplétion CD4+ ou à une diminution du DAS28, et (ii) que la diminution du DAS28 était doublée en présence de déplétion des CD4+ comparé à son absence, et (iii) des concentrations plus élevées de rituximab étaient liées à une meilleure réponse clinique. - Dans les AAV, la relation entre les concentrations de rituximab et les niveaux d'ANCA a été décrite à l'aide d'un modèle de transit semi-mécanistique avec rétrocontrôle négatif. Ce modèle a montré que (i) la diminution des niveaux d'ANCA induite par le rituximab était profonde mais retardée et plus soutenue chez les patients avec MPO-ANCA que chez ceux avec PR3-ANCA, et (ii) des concentrations plus élevées de rituximab étaient associées à une diminution plus importante des niveaux d'ANCA. Des administrations répétées de rituximab seraient susceptibles d’améliorer la réponse clinique au rituximab et diminuer le risque de rechute. En conclusion, ce travail a été le premier à montrer une PK non linéaire du rituximab dans une maladie auto-immune (AAV), et à quantifier la relation complexe entre la déplétion des cellules B induite par le rituximab, la diminution des CD4+, et son efficacité clinique
Rituximab is a chimeric IgG1 monoclonal antibody (mAb) that targets CD20, a protein on the surface of most B lymphocytes. It is approved as a second line treatment in rheumatoid arthritis (RA) patients, and is used in anti-neutrophil cytoplasmic antibody (ANCA)-associated vasculitis (AAV). There is a large interindividual variability in rituximab pharmacokinetics (PK), and its concentration–response relationship. Rituximab binds to CD20 with high affinity and specificity and form mAb-target complexes which are eliminated by immune system. This elimination is usually described using target-mediated drug disposition (TMDD) models. For rituximab, TMDD was never reported in autoimmune inflammatory diseases, as RA or AAV. This PhD work aimed at studying the variability of PK and cconcentration-response relationship of rituximab using population PK and pharmacokinetic-pharmacodynamic (PK-PD) modeling. This work was done using data from : - 52 RA patients of the rheumatology department of Tours University Hospital, where rituximab concentrations, CD4+ counts (biomarker) and disease activity score in 28 joints (DAS28, clinical response) were measured. - 92 AAV patients included in the RAVE trial (Rituximab for AAV), where rituximab concentrations, antibodies to proteinase 3 (PR3-ANCA), and antibodies to myeloperoxidase (MPO-ANCA) (biomarkers) were measured. In RA patients, rituximab PK was described using a two-compartment model with linear (endogenous) elimination. No target-elimination of rituximab or influence of B-cell count was detected. This may be due to (i) a low amount of target antigen compared to B-cell neoplasia, and/or (ii) insufficiently dense PK data. In AAV patients, nonlinear target-mediated elimination was detected at the beginning of the follow-up. A simplified TMDD model was used, where target was modeled as a latent variable, and irreversible binding to rituximab on its target was assumed. Latent variable may be partly interpreted as the fraction of CD20 (circulating or present at the B-cell membrane) available for rituximab binding. The negligible target-mediated elimination towards the end of the follow-up in RA and AAV may be due to the sustained B-cell depletion after rituximab treatment. Rituximab-induced B cell depletion was shown to alter count and function of other immune cells. However, quantitative relationship between depletion of blood B cells, immune cells, and clinical response in both RA and AAV remain unclear. In addition, this relationship, highly variable among patients, was never quantified using PK-PD modeling. In RA patients, the relationship between rituximab concentrations and CD19+ counts, between CD19+ and CD4+ counts, and between CD4+ counts and DAS28 (clinical activity score in RA) was described using cell lifespan, indirect response and direct Emax models, respectively. This study showed that (i) the amplitude of CD19+ count depletion was not associated with CD4+ decrease or DAS28, and (ii) CD4+ decrease leads to two-fold DAS28 decrease compared to no CD4+ decrease, and (iii) higher rituximab concentrations were related to a better clinical improvement. In AAV patients, the relationship between rituximab concentrations and ANCA levels was described using a semi-mechanistic transit model with negative feedback. This model showed that (i) rituximab-induced decrease of ANCA levels was deep but delayed, and more sustained in patients with MPO-ANCA than in those with PR3-ANCA, and (ii) higher rituximab concentrations were associated with deeper decrease of ANCA levels. Moreover, repeated rituximab courses may improve clinical response to rituximab, and increase the time to disease relapse. Overall, this work was the first to report nonlinear PK of rituximab in autoimmune disease (AAV), and to quantify the complex relationship between rituximab-induced B-cell depletion, CD4+ decrease, and the clinical response
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16

Wright, Tracey Jane. "Characterisation of CD23 cleavage by endogenous and exogenous proteases using neo-epitope antibodies". Thesis, University of Leicester, 2000. http://hdl.handle.net/2381/29820.

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CD23 is the low affinity IgE receptor. It is a type II integral transmembrane glycoprotein that can be shed from the cell surface forming soluble products of approximately 37, 33, 29, 25 and 16kDa. It appears that membrane and soluble CD23 have opposing regulatory functions and that inhibition of CD23 shedding may have potential to alleviate both allergic and inflammatory diseases. This has focused attention on the endogenous protease(s) responsible for CD23 shedding, leading to the demonstration that both the 37 and 33kDA sCD23 fragments are cleaved from the cell surface by a metalloprotease. In order to characterise the cleavage events within CD23, anti-neoepitope antibodies specific for the newly created amino and carboxy termini of the two predominant cleavage sties within CD23 (producing the 37 and 25kDa soluble CD23 products) were raised. Characterisation of these antibodies demonstrated that the proteolytic cleavage events responsible for creating the 37 and 25kDa sCD23 fragments are independent of each other. Furthermore, two different proteases were shown to be responsible for cleaving these two fragments. The work described in this thesis confirms previous reports that 37kDA sCD23 is cleaved by a metalloprotease, however cleavage of the 25kDa fragment was not inhibited by metalloprotease inhibitors. The production of the two different sized sCD23 molecules by different proteases has important implications for targeting the proteolytic cleavage events to alleviate symptoms of allergic and inflammatory diseases. This emphasises the importance of defining the biological functions of mCD23 and each of the sCD23 molecules.
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17

Heath, Andrew. "Assessment of anti- CD40 monoclonal antibodies as novel immunological adjuvants in conjugate vaccines". Thesis, University of Sheffield, 2008. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.500260.

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18

Prasad, Vijay Narayana Sharma Bhagawati. "Assessment of Anti-CD40 Monoclonal Antibodies as Novel Immunological Adjuvants in Conjuate Vaccines". Thesis, University of Sheffield, 2008. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.500680.

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19

Geldart, Thomas Richard. "Efficacy and toxicity of anti-CD40 monoclonal antibodies in the treatment of malignancy". Thesis, University of Southampton, 2004. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.403845.

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20

Chan, Ka-kui. "Molecular mechanisms of IL-2 mediated BCL10 nuclear localization and the therapeutic role of an anti-CD25 antibody in nasal NK-cell lymphoma". Click to view the E-thesis via HKUTO, 2009. http://sunzi.lib.hku.hk/hkuto/record/B4218244X.

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21

Felonato, Maíra. "Importância da molécula CD28 (molécula co-estimulatória de linfócitos T) na Paracoccidioidomicose pulmonar". Universidade de São Paulo, 2007. http://www.teses.usp.br/teses/disponiveis/42/42133/tde-08012008-132539/.

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Como a imunoproteção na Paracoccidioidomicose (PCM) é principalmente mediada por células T, investigamos o impacto da deficiência de CD28, molécula co-estimulatória de linfócitos T, na gravidade da infecção primária e secundária pelo Paracoccidioides brasiliensis. Quando comparados a camundongos C57Bl/6 normais (WT), camundongos CD28-deficientes (CD28KO) apresentaram infecção mais grave associada à produção diminuída de anticorpos e citocinas. Além disso, a pré-imunização de animais deficientes e normais resultou em imunoproteção equivalente. Inesperadamente, a sobrevida de animais CD28KO foi significativamente maior que a dos WT, apesar da sua elevada carga fúngica tecidual. Em conclusão, nosso trabalho mostrou que a deficiência de CD28 resulta em PCM mais grave, porém não letal, associada a resposta imune deficiente. Além disso, verificamos que carga fúngica elevada, na ausência da imunidade adaptativa efetora, não ocasiona diminuição de sobrevida, revelando que a resposta imune na PCM pode tanto proteger como ser deletéria aos hospedeiros.
As immunoprotection in Paracoccidioidomycosis (PCM) is mainly mediated by T cells, and CD28 is a costimulatory molecule for T lymphocytes, we investigated the influence of CD28 deficiency in primary and secondary PCM. Compared with normal C57BL/6 mice, CD28-deficient (CD28KO) mice developed a more severe infection associated with impaired antibody and cytokine production. In addition, CD28KO and WT mice previously immunized by the s.c. route developed equivalent immunoprotection when challenged by the pulmonary route. Interestingly, CD28KO mice presented increased mean survival time despite their elevated fungal loads in the lungs. In conclusion, our work showed, for the first time, that CD28-deficiency results in more severe, but not overwhelming, PCM. Furthermore, in the absence of effector adaptative immunity, elevated fungal loads do not cause lethal infections, revealing the protective and deleterious effects of immune responses to Paracoccidioides brasiliensis infected hosts.
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22

Sandin, Linda. "Immunomodulatory Therapy of Solid Tumors : With a Focus on Monoclonal Antibodies". Doctoral thesis, Uppsala universitet, Klinisk immunologi, 2013. http://urn.kb.se/resolve?urn=urn:nbn:se:uu:diva-210080.

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Cancer, historically considered a genetic disease, is currently acknowledged to affect the whole body. Our immune system is one key player that can elicit a response against malignant cells but can also promote tumorigenesis. Tumors avoid immune recognition by creating a suppressive microenvironment and inducing tolerance. T-cells are regarded a major effector cell type in tumor immunotherapy. An important ”switch” needed for T-cell activation involves so-called costimulatory and coinhibitory receptors. In this thesis, experimental tumor models were used to investigate the potential of immunomodulatory antibodies to stimulate immune cells and subsequently eliminate tumors. First, systemic antibody blockade of two negative checkpoint regulators (CTLA-4 and PD-1) present on T-cells was evaluated in combination with local CpG therapy or standard BCG treatment. Indeed, this combinatorial therapy with CpG augmented anti-tumor effects with increased levels of tumor-directed T-cells and reduced tumor-infiltrating Tregs. Secondly, as these immunomodulatory antibodies elicit severe side effects in patients, a local low-dose delivery regimen was explored as an alternative to systemic bolus treatment. Our results demonstrated that an approximately seven times lower dose of aCTLA-4, compared to systemic delivery, could eradicate both primary and distant tumors. CD40-expressing APCs are another potential target in antibody-mediated cancer therapy. CD40-stimulated dendritic cells (DCs) have the capability to activate tumor-directed T-cells to kill tumor cells. We next sought to investigate agonistic CD40 antibody efficacy and in vivo biodistribution when delivered locally compared to the equivalent systemic dose. Anti-tumor effects were dependent on CD8+ T-cells, host CD40 expression and the presence of tumor antigen at the injection site. CD40 antibodies were cleared from the circulation and accumulated in lymphoid organs, where, upon repeated aCD40 dosing, target APC populations increased in numbers and upregulated their surface CD40 expression. Lastly, CD40 agonist antibodies were mixed with nanoparticles to enhance their stimulatory properties. B-cells demonstrated increased proliferative capacity and DCs became more activated when exposed to the cocktail. Further, this combination reduced serum levels of pro-inflammatory cytokines compared to plain antibodies.       The results herein advocate further exploratory studies of the delivery of monoclonal antibodies at the tumor site in order to improve anti-tumor effects and reduce toxicity.
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23

Salgado, Rafael Moysés. "Avaliação do papel do soro imune de camundongos CD28KO (deficiente em IgG especifica) na interação in vivo e in vitro do T. cruzi Sylvio X10/4 com células da linhagem macrofágica". Universidade de São Paulo, 2014. http://www.teses.usp.br/teses/disponiveis/42/42133/tde-11072014-135353/.

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As células da linhagem macrofágica são fundamentais na infecção por T. cruzi. Além do reconhecimento por PRRs, a interação com anticorpos e/ou complemento facilita a internalização. Avaliamos o papel in vivo e in vitro de IgM e IgG específicas na saída de parasitas Sylvio X10/4 do sangue, um clone miotrópico de T. cruzi que causa infecção sem parasitemia patente. Devido à sua saída espontânea, estudamos a remoção no sexto dia de infecção, momento em que a parasitemia subpatente aumenta. Camundongos foram infectados e tratados com soro normal (NMS), soro crônico (B6) e soro de animais CD28KO crônicos (que produzem somente IgM). O grupo tratado com soro de CD28KO apresentou uma remoção significativa, porém menos eficiente do que com soro crônico (B6). Tais resultados foram reproduzidos em estudo in vitro na invasão de macrófagos (derivados de medula óssea ou do peritônio) com os distintos tratamentos. Concluímos que os macrófagos são fundamentais na remoção dos parasitas e os anticorpos, não somente IgG, mas também os da classe IgM reforçam este processo.
The cells of the macrophage lineage are essential for the infection by T. cruzi. Besides the recognition by PRRs, interaction with antibodies and/or complement facilitates internalization. We evaluated the role in vivo and in vitro of specific IgM and IgG in the blood output of parasites Sylvio X10/4, clone myotropic of T. cruzi which causes infection without patent parasitemia. Due to its spontaneous exit, we studied the removal on the sixth day of infection, when the parasitemia subpatent increases. Mice were infected and treated with normal mouse serum (NMS), chronic serum (B6) and serum from CD28KO chronic mice (which produce only IgM). The group treated with CD28KO serum showed a significant removal, but less efficiently than with chronic serum (B6). These results were reproduced in vitro study on the invasion of macrophages (derived from bone marrow or peritoneum) with these different treatments. We conclude that macrophages are essential in the removal of parasites and antibodies, not only IgG, but also IgM enhance this process.
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24

Chan, Ka-kui y 陳家駒. "Molecular mechanisms of IL-2 mediated BCL10 nuclear localization and the therapeutic role of an anti-CD25 antibody in nasal NK-celllymphoma". Thesis, The University of Hong Kong (Pokfulam, Hong Kong), 2009. http://hub.hku.hk/bib/B4218244X.

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25

PIEVANI, ALICE SILVIA. "Cytokine-induced killer (cik) cell cultures for the adoptive immunotherapy of hematological malignancies: characterization and new therapeutic strategies for clinical application". Doctoral thesis, Università degli Studi di Milano-Bicocca, 2011. http://hdl.handle.net/10281/20178.

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Cytokine-induced killer (CIK) cells are a heterogeneous population of lymphocytes obtained in vitro within 21 days from mononuclear cells under the influence of cytokines. CIK cells show potent MHC-unrestricted cytotoxicity against a variety of tumor cells, in particular hematological malignancies, and minimal tendency to induce graft-versus-host disease. The expanded bulk CIK culture consists of over 90% CD3+ cells, of which the majority coexpress CD56 and the remaining cells are CD56-. CD3+CD56+ “true” CIK cells are terminally differentiated non dividing lymphocytes which could deliver potent MHC-unrestricted cytotoxicity for the immediate destruction of tumor cells. The other less cytotoxic CD3+CD56- cell subset represents a progenitor reservoir that could proliferate and differentiate into CD3+CD56+ CIK cells. CD3+CD56+ CIK cells express activating NK receptors including NKG2D, DNAM-1 and low levels of NKp30. Cell signalling not only through TCR/CD3, but also through NKG2D, DNAM-1 and NKp30, leads to CIK cell activation resulting in granule exocytosis and cytotoxicity. Antibody blocking experiments revealed that NKG2D, DNAM-1 and NKp30 are actually involved in tumor cell recognition and killing. Anti-CMV specific CIK cells could be expanded in standard CIK conditions and mediate both specific, MHC-restricted recognition of a CMV-pulsed autologous target and NK-like non specific cytolytic activity against leukemic cell targets. Antibody blocking of NKG2D and NKp30 only inhibited NK-like cytotoxicity. Their dual effector function suggests that CIK cells, when used in a clinical setting, may control both neoplastic relapses and viral infections, two frequently associated complications in transplanted patients. B-cell non-Hodgkin lymphoma is only partially susceptible to CIK-mediated lysis. The addition of anti-CD20 monoclonal antibodies GA101 or rituximab increased cytotoxicity mediated by CIK cell cultures by 35% and 15%, respectively. This enhancement was mainly due to antibody-dependent cytotoxicity mediated by the 1%-10% NK cells contaminating CIK cultures. The addition of human serum inhibited NK-cell activation induced by rituximab, but not activation induced by GA101. Overall lysis in presence of serum, even of a resistant B-NHL cell line, was significantly increased by 100 mcg/mL of rituximab, but even more so by GA101, with respect to CIK cultures alone. The combined use of CIK cells with anti-CD20 mAbs could represent a novel immunotherapy protocol for the treatment of B lymphoma patients with resistant disease.
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26

Prampero, Anna Carolina. "Produção de anticorpos monoclonais anti-GITR e anti-CD25 através de cultivo de hibridomas e comparação do seu potencial como agentes antitumorais". Universidade Federal de São Carlos, 2017. https://repositorio.ufscar.br/handle/ufscar/9210.

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Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)
Nowadays, cancer is one of the most feared diseases, affecting each day more and more people worldwide. The importance of new cancer treatment researches is very clear since the ones that has been used are not very effective and may lead to drug resistance, implying in a constant dose increasing which can lead to toxicity issues. Collateral effects and the instability generated in the patient’s organism are also reasons why the necessity of discovering new cancer treatments is imminent. A treatment alternative that has aroused interest is the use of monoclonal antibodies as immunotherapics, since they act by stimulating the patient’s immune system neutralizing the tumor cells in a very efficient and specific way. This kind of antibody can be produced by culturing hybrid animal cells, better known as hybridoma, under strictly controlled conditions so they can be studied and used in human beings. For this reason, the major goal of this project was the production of murine monoclonal antibodies using hybridoma cell culture in order to stablish an efficient culture methodology for hybridomas PC-61 or DTA1 producers of monoclonal antibodies anti-CD25 and anti-GITR, respectively, with high quality and enough amounts using Fetal Bovine Serum (FBS) free medium to, in the future, carry out animal model studies of their potential as therapeutic agents for cancer treatment. Both hybridomas were cultivated on a small scale with RPMI medium and addition of SFB, for comparative purposes and only one was selcted for the second step. The sequential adaptation methodology test, consisted in a gradual percent’s reduction of medium with serum at the same time that increase the percentage of commercial medium without serum, and was selected the medium without SFB in which the hybridoma was better adapted. After was carried out on a laboratory scale in a system type spinner flask (500 ml) with the commercial medium selected in the previous step, in controlled conditions of temperature (37 ° C) and pH (7.2). Based on analyzes of cell culture results, amino acid consumption and monoclonal antibodies quantification , SFM commercial medium SFB-free provided better results for culturing the PC-61 hybridoma, allowing the pilot scale culture reached even higher cell densities than in the standard medium with addition of FBS.
O câncer é uma das doenças mais temidas da atualidade, e atinge cada vez mais pessoas em todo o mundo. A importância de pesquisas sobre novos tratamentos na luta contra o câncer é clara e consensual, uma vez que os que vem sendo utilizados, não são muito eficientes, causam resistência à medicação utilizada o que implica na utilização de doses crescentes que por sua vez podem gerar problemas de toxicidade. Os efeitos colaterais e a instabilidade gerada no organismo do paciente, também são fatores da necessidade de pesquisar novos caminhos para o tratamento do câncer. Uma das alternativas de tratamento que tem despertado interesse é a utilização de anticorpos monoclonais (mAbs) como imunoterápicos, os quais agem estimulando o próprio sistema imune do paciente neutralizando a ação das células tumorais de forma eficiente e específica. A produção de tais anticorpos pode ser feita mediante o cultivo de células animais híbridas, mais conhecidas como hibridomas, sobre condições estritamente controladas para que possam ser estudados e utilizados em humanos. Por essa razão definiu-se como objetivo desse trabalho a produção anticorpos monoclonais murinos por meio de cultivo de hibridomas com a finalidade de estabelecer uma metodologia eficiente de cultivo dos hibridomas PC-61 ou DTA1 secretores dos mAbs anti-CD25 e antiGITR respectivamente, com qualidade e em quantidades suficientes utilizando meios livres de soro fetal bovino (SFB), para a seguir efetuar estudos em modelo animal de seu potencial como agentes terapêuticos no tratamento de câncer. Os dois hibridomas foram cultivados em pequena escala utilizando meio RPMI-1640 e adição de SFB, para fins comparativos e somente um foi selecionado para a próxima etapa. O teste da metodologia de adaptação sequencial, onde houve a redução gradativa da porcentagem de meio RPMI-1640 com 10% de SFB e o aumento da porcentagem de meio comercial sem SFB, e foi selecionado o meio livre de SFB em que o hibridoma melhor se adaptou. Posteriormente foi realizado o cultivo do hibridoma em escala laboratorial em sistema de frasco agitado biorreator do tipo Spinner (500 mL) com o meio livre de SFB selecionado na etapa anterior, sob condições bem controladas de temperatura (37ºC), pH (7,2). Com base nas análises dos resultados dos cultivos celulares, metabolismo de aminoácidos e quantificação de mAbs, o meio comercial SFM livre de SFB proporcionou melhor resultados para o cultivo do hibridoma PC-61, permitindo que o cultivo em escala laboratorial atingisse densidades celulares ainda maiores que no meio padrão com adição de SFB. Como consequência desse vasto crescimento celular em quantidades abundantes de mAbs foram conseguidas para iniciar num futuro próximo ensaios em modelos animais.
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27

Kennedy, Adam David. "Enhancing rituximab therapy : analyzing the interaction between rituximab and the human complement pathway /". 2005. http://wwwlib.umi.com/dissertations/fullcit/3189294.

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André, Ana Filipa Santos. "Selection of single domain antibodies against the CD20 receptor: a new treatment with potencial anti-tumor properties for B-cell malignancies". Master's thesis, 2016. http://hdl.handle.net/10451/25211.

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Tese de mestrado, Biologia Molecular e Genética, Universidade de Lisboa, Faculdade de Ciências, 2016
Lymphoma is the third most common neoplasia in the world. Within lymphomas, non-Hodgkin lymphoma (NHL) is the most common affecting mainly B cells. For more than three decades, chemotherapy and radiotherapy have been the only treatments available, but since the discovery of Rituximab, a new era of lymphoma therapy was inaugurated, once it was the first monoclonal antibody approved against the CD20 receptor. The CD20 receptor is an antigen expressed on the B-cells surface, and it is present nearly in all of its maturational development, being absent only in the stages of the pro-B lymphocyte and plasma cells. Furthermore, the CD20 receptor is also present on >90% of the B-cell NHL. These characteristics make this receptor an ideal target for immunotherapy. Besides the success of Rituximab, various mechanisms of resistance have been developed by the tumoral cells against this antibody, such as the decrease of the CD20 expression on B-cells, immunogenicity, structural changes affecting the binding region of the CD20 antibody or alterations in the cell membrane. New anti-CD20 antibodies have been developed to overcome the disadvantages of Rituximab, such as Ofatumumab and Obinutuzumab, presenting a different immunogenicity and binding to the different epitopes on the target with a different affinity. Apart from the progress in the lymphoma therapy, a significant population of patients still succumbs to this disease, as tumoral cells are always changing, making the search for better antibodies a never-ending process. Thus, the aim of this project consisted in the development and characterization of a new antibody against the CD20 receptor. To achieve this goal, the potential of rabbit derived single-domain antibodies (sdAbs) as therapeutic molecules were explored. For that, one rabbit was immunized with the CD20 receptor and an immune VH and VL sdAb library was generated. Then, a subtractive cell phage display screening was used for antibody selection. This approach allowed a specific selection of one sdAb in the VL format against the CD20 receptor in cells. In summary, the strategy explored in the present project resulted in an antibody that, according to its characteristics, could be a promising candidate in the treatment of NHL and other B-cell malignancies.
Os linfomas são a terceira neoplasia mais comum no mundo, sendo os linfomas não-Hodgkin os mais frequentes. Dentro dos linfomas não-Hodgkin, cerca de 85-90% são de células B. Os linfomas desenvolvem-se maioritariamente a partir dos nódulos linfáticos, no entanto podem formar-se a partir de qualquer outro tecido. Durante mais de três décadas, os únicos tratamentos disponíveis para esta doença eram a quimioterapia e a radioterapia. No entanto, com a descoberta do Rituximab, um anticorpo específico para o recetor CD20 presente nos linfomas de células B, começou uma nova era no campo das imunoterapias. O anticorpo Rituximab, uma vez que foi o primeiro a ser descoberto, faz parte da primeira geração de anticorpos anti-CD20. Este é um anticorpo quimérico, uma vez que é constituído por um IgG1 glicosilado composto por uma região constante kappa humana e regiões variáveis leves e pesadas murinas. Este anticorpo atua essencialmente através de três principais mecanismos de ação: citotoxicidade mediada por anticorpos (ADCC); citotoxicidade dependente do complemento (CDC) e indução da apoptose. O recetor CD20 é uma molécula expressa na superfície das células B e está presente na maioria das fases de maturação destas células, com exceção da fase de linfócitos pró-B e nas células plasmáticas. Para além disso, está presente em mais de 90% dos linfomas não-Hodgkin de células B. No entanto, apesar da sua função ainda não ser totalmente conhecida, pensa-se que possa estar envolvido no fluxo de cálcio. Este recetor é uma fosfoproteína não glicosilada com 4 domínios membranares: os domínios N e C terminal que são intracitoplasmáticos e 2 loops adicionais que são extracelulares. Devido a estas suas características, o recetor CD20 é considerado um bom alvo para imunoterapias, nomeadamente terapias para linfomas não-Hodgkin de células B. Apesar do sucesso do Rituximab, têm vindo a ser descritos vários mecanismos de resistência das células tumorais contra este anticorpo, nomeadamente a diminuição da expressão de CD20, mudanças estruturais que afetam o local de ligação do anticorpo à molécula ou alterações na membrana da célula, o que diminuiu a sua eficácia. Este aspeto fez com que fosse necessária a contínua procura por novos anticorpos para colmatar as lacunas do Rituximab. Assim, ao longo dos anos, foram descobertos novos anticorpos específicos para CD20, como o Ofatumumab e o Obinutuzumab, que têm uma diferente imunogenicidade e reconhecem diferentes epítopos na molécula CD20 aos quais se ligam com diferentes afinidades, atuando assim com diferentes mecanismos de ação. Ainda assim, este tipo de doença continua a afetar imensas pessoas, muitas vezes não existindo um tratamento eficaz devido às múltiplas resistências das células tumorais. Tendo em conta este contexto e uma vez que os anticorpos disponíveis no mercado não conseguem resolver estes problemas, a procura por novos anticorpos mais vantajosos continua. Atendendo a esta necessidade, o objetivo deste projeto é o desenvolvimento e caracterização de um anticorpo de pequeno domínio específico para CD20. Os anticorpos de pequenos domínios têm várias vantagens em relação aos IgGs completos, principalmente devido ao seu reduzido tamanho, que faz com que estes anticorpos tenham melhor acesso ao alvo na superfície da célula, para além disso podem ainda ser facilmente expressos em bactérias como proteína. Têm ainda a vantagem, como moléculas terapêuticas, de serem mais estáveis em circulação que os anticorpos completos. Estas características permitem uma administração de maiores quantidades por grama de produto, o que leva a um aumento significativo da potência por dose e na redução do custo de produção. Para o desenvolvimento do projeto, inicialmente foi imunizado um coelho com o péptido CD20 e com células HEK 293T transfetadas com o recetor CD20. Antes de cada imunização, o soro era recolhido para ser avaliado através de ELISA. Ao dia 89, quando foi atingido um elevado título de anticorpos, procedeu-se à recolha do soro final e à eutanásia do coelho. Os ensaios de ELISA permitiram confirmar que o soro extraído após as imunizações estava a reconhecer não só as células Raji, que contêm à sua superfície CD20, mas também o péptido CD20, por outro lado o soro recolhido antes das imunizações não reconhecia nem as células Raji, nem o péptido. Após a eutanásia, foram recolhidos o baço e a medula que são os órgãos onde se encontra um maior número de células plasmáticas que produzem anticorpos. A partir destes órgãos, procedeu-se à extração de ARN usando o reagente Tri. A partir do ARN extraído foi possível sintetizar a primeira cadeia de ADN. O cADN sintetizado foi utilizado para a construção de bibliotecas imunes de pequenos domínios de anticorpos específicos para o recetor CD20, através da amplificação por PCR das famílias de cadeias variáveis leves e pesadas. Esses produtos resultantes da amplificação foram clonados no vetor pComb3x, que é necessário na técnica de phage display, resultando numa biblioteca imune com uma grande diversidade, ideal para este tipo de seleção. Em seguida, as bibliotecas resultantes foram selecionadas através da tecnologia de phage display que permite a seleção de anticorpos específicos para CD20 em células que contenham esse recetor. Esta tecnologia baseia-se na engenharia genética de bacteriófagos e em várias rondas de seleção contra o antigénio e propagação dos fagos. Resumidamente, os fagos vão conter à sua superfície o fenótipo correspondente ao genótipo encapsulado no seu interior que contem a sequência correspondente aos fragmentos de ADN obtidos através da construção das bibliotecas de anticorpos. Seguem-se várias rondas de seleção onde vão sendo eliminados os anticorpos-fagos que não se ligam ou que possuem uma fraca ligação às células que contêm o antigénio, neste caso o recetor CD20, através de várias lavagens. Estas rondas vão sendo repetidas até obtermos uma população de anticorpos específica para o alvo. Para este phage display, foram utilizados 3 tipos de células: células Raji, que está descrito que expressam o CD20, pois são células de linfoma B; células HEK 293T que não expressam CD20 e por isso foram utilizadas para eliminar os anticorpos não específicos para este recetor; células Jurkat, que tal como as anteriores não possuem CD20, pois tratam-se de células T de leucemia aguda e que por isso foram também utilizadas para eliminar anticorpos não específicos. Esta seleção resultou num conjunto de anticorpos-fagos específicos para o recetor CD20, resultado que foi confirmado através de Western Blot. Após a seleção por phage display, foi necessário fazer uma seleção em larga escala para avaliar os anticorpos que melhor eram expressos e que melhor se ligavam ao alvo. Para esta avaliação da expressão foi necessário clonar o ADN resultante dos fagos selecionados por phage display, num outro vetor que permitisse a expressão de proteína, neste caso o vetor pT7-PL. Esta avaliação da ligação e expressão foi feita através de ensaios de ELISA com extrato proteico de células Raji e células Raji. Para além disso, após várias seleções os melhores 10 clones foram sequenciados para avaliar a homologia entre si e verificar os CDRs. Através do alinhamento da sequência de aminoácidos obtida a partir da sequenciação, verificou-se que 9 dos clones eram iguais, restando assim apenas 2 clones. A especificidade dos dois clones selecionados para o recetor CD20 foi avaliada através de Western Blot, sendo que um deles (anticorpo no formato VL) era específico para o recetor pretendido. Estas metodologias levaram à seleção de um anticorpo de pequeno domínio específico para CD20, que devido às suas características únicas e diferentes dos que já existem no mercado poderá ser um promissor candidato para ser usado como agente terapêutico para linfomas de células B que expressem o recetor CD20.
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29

PIGHI, CHIARA. "Impact of anti-CD20 tumor-targeting therapeutic monoclonal antibodies on human Natural Killer cell responsiveness and plasticity: relevance of FcgammaRIIIA/CD16 affinity ligation conditions". Doctoral thesis, 2018. http://hdl.handle.net/11573/1116013.

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My study is focused on understanding the mechanisms underlying the modulation of NK cell responsiveness and plasticity induced by tumor targeting therapeutic anti-CD20 monoclonal antibodies (mAbs) nowadays routinely used in the treatment of B-cell malignancies and autoimmune disorders. Anti-CD20 mAbs are grouped into type I and II subtypes. Type I mAbs induce CD20 redistribution into lipid rafts and display a remarkable ability to activate complement-dependent cytotoxicity (CDC). On the other hand, type II mAbs, which are not able to localize CD20 complexes into lipid rafts and induce weak or no CDC, evoke more homotypic adhesion and direct killing of target cells. Both type I and II mAbs demonstrate efficient phagocytosis and antibody-dependent cytotoxicity (ADCC). Natural Killer (NK) cell-mediated ADCC, based on the recognition of IgG-opsonized targets by the low affinity Fc receptor for IgG FcgammaRIIIA/CD16, represents one of the main mechanisms by which anti-CD20 mAbs mediate their anti-tumor effects. Besides ADCC, CD16 ligation also results in the production of cytokines such as IFN-gamma that plays a key role in the shaping of adaptive immune responses. Rituximab is a chimeric type I anti-CD20 mAb of 1st generation and is considered the reference molecule for the comparison with new generation anti-CD20 mAbs, designed to optimize clinical efficacy. Among them, obinutuzumab is a humanized Fc-glycoengineered type II anti-CD20 mAb of 3rd generation designed to increase the affinity for CD16 receptor and consequently the killing of mAb-opsonized targets. However, the impact of CD16 ligation in optimized affinity conditions on NK functional program is not completely understood. Herein, I demonstrated that CD16 affinity ligation conditions may dictate both the amplitude of NK responsiveness (cytotoxicity and IFN-gamma production) as well as the ability to shift the NK functional program. Indeed, I observed that the interaction of NK cells with obinutuzumab-opsonized targets results in enhanced cytotoxicity and IFN-gamma production as compared with the parental non-glycoengineered mAb or the reference molecule rituximab, independently from the CD16-158V/F allotype. The affinity ligation conditions also strictly correlate with the ability to induce CD16 surface down-modulation and lysosomal targeting of receptor-coupled signaling elements. Indeed, a preferential degradation of FcepsilonRIgamma chain and Syk tyrosine kinase was observed upon obinutuzumab stimulation independently from the CD16-158V/F allotype. Notably, although the down-regulation of FcepsilonRIgamma/Syk module hesitates in the impairment of cytotoxic function induced by CD16, NKp46 and NKp30 activating receptors, obinutuzumab-experienced NK cells exhibit an increased ability to produce IFN-gamma in response to cytokines and target stimulation as well as to obinutuzumab-mediated CD16 re-stimulation. Relying on the observation that obinutuzumab-experienced NK cells, under molecular and functional profile, resemble the distinctive features of the long-lived and highly functional “memory” NK cells, a population recently identified in HCMV seropositive individuals, I assessed the capability of anti-CD20 mAbs to affect the expansion as well as the phenotypic and functional properties of the “memory” NK subset. My data show that the majority of the analysed healthy donors is HCMV seropositive and exhibits a detectable population of “memory” NK cells (CD3- CD56+ FcepsilonRIgamma- CD16+) accounting for 3 to 50% of peripheral blood NK cells. I observed that “memory” NK cells selectively undergo 2- to 12-fold expansion upon co-culturing with anti-CD20-opsonized targets; on the opposite, the proliferation of “conventional” NK cells (CD3- CD56+ FcepsilonRIgamma+ CD16+) is not affected by CD16 stimulation. I also noted that anti-CD20 mAb in vitro expanded “memory” NK cells show the molecular and functional hallmarks of their freshly isolated counterpart, including the increased expression of NKG2C receptor, the reduced expression of NKp46 receptor associated to an enhanced functional activity in response to CD16 re-stimulation, particularly in terms of IFN-gamma production.
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30

Crank, Michelle C. "Understand the mechanism of action of Rutuximab® in the reversal of multidrug resistance in a Non-Hodgkins Lymphoma cell line". 2006. http://edissertations.library.swmed.edu/pdf/CrankM030206/CrankMichelle.pdf.

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31

Lemos, Francisca Mendes. "Adverse events/mode of action relationship of monoclonal antibodies-based therapies : overview of marketed produts in the European Union". Master's thesis, 2014. http://hdl.handle.net/10451/18333.

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Tese de mestrado, Ciências Biofarmacêuticas, Universidade de Lisboa, Faculdade de Farmácia, 2014
In the past few years, great discoveries and improvements have been done in drug development field and a market that was previously populated just by chemical drugs is now growing to include the so called biopharmaceuticals. As biotechnologically-derived drugs rely on the fundamental understanding of the related disease, it can be predicted that they will play a major – if not dominant – role in the drug development arena of the next decades. Following the success of recombinant proteins, therapeutic Monoclonal Antibodies (mAbs) represent the second wave of innovation created by the biotechnology industry. Overcoming the problems initially raised by these biopharmaceuticals, the recent generations of mAbs have managed to reduce some of the immunogenicity problems observed with murine mAbs. Other concerns remain, however, and the adverse events arising during the long-life experience will continue to be an important factor to monitor. The target specificity of mAbs associated to the fact that they are large protein molecules make the emergence of off-target or metabolite–related toxicities less probable, being immunogenicity and target-mediated effects the most relevant determinants of toxicity. This project focus was in the correlation and comparison of mAbs’ adverse events with their specific mechanism of action. The data here analysed comprises mainly European data (EMA) but also some United States data [1]. Due to the large diversity of mechanisms for the marketed mAbs, the analysis has been restricted to three pharmacological classes of mAbs: anti-TNFα, anti-VGEF and anti-CD20 mAbs. Adverse events were compared within each mAb class and then compared through all mAbs classes. There were antibody-related adverse events reported transversally for all mAbs but there were also some class-related adverse events which were only reported in specific classes, with specific mechanisms of action. For class-related adverse events it was observed that additional key factors – like administration routes, mAbs structural configurations and profile of patients receiving those mAbs – may also impact the adverse events and cannot be excluded in safety profile characterisation. It was confirmed that the adverse events reported for all mAbs analysed were strictly related to mAbs’ mechanism of action. Hence, characterisation of each mAb specifities together with a precise understanding of the mAbs mechanism of action is crucial for mAbs safety profile characterisation.
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32

Chang, Chu-Ting y 張筑婷. "Study of Natural Products from Cinnamomum kotoense, Arctium lappa and Agave sisalana Regulation Human T Lymphocytes Immune Responses Induced by Anti-CD3 and Anti-CD28 Antibodies". Thesis, 2008. http://ndltd.ncl.edu.tw/handle/47963629530302964174.

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碩士
輔仁大學
生命科學系碩士班
96
The immune system is a collection of mechanisms within an organism that protects against disease by identifying and killing pathogens and tumor cells. However, overactive effector immune responses to autologous or allogeneic antigens can result in immune-mediated diseases such as hypersensitivity and autoimmune diseases. One of the therapeutic objectives in autoimmune diseases is blocking of activation, proliferation and cytokine production in T lymphocytes. There are immunosuppressive drugs used for autoimmune diseases, but they almost accompany with serious side effects. Therefore, we attempted to identify other immunomodulators from natural products that could be as an adjuvant treatment for autoimmune diseases. The previous data indicated that the natural products kaempferol 3-O-a-L-[2,4-di-(E)-p-coumaroyl] rhamnopyranoside (C39H32O14; MW=724; K3), arctigenin (C21H24O6; MW=372; AC), and (±)-3,9-dihydroeucomin (C17H16O5; MW=300; DC) isolated from Cinnamomum kotoense, Arctium lappa and Agave sisalana, respectively, inhibited human peripheral blood mononuclear cells (PBMC) proliferation stimulated by phytohemagglutinin (PHA). In the present study, human T lymphocytes were purified from PBMC and used as target cells. The regulation of K3, AC, and DC in human T lymphocytes immune responses induced by anti-CD3 and anti-CD28 antibodies (anti-CD3/CD28 Abs) was studied. The results indicated that (1) Primary human T lymphocytes has been isolated from PBMC by nylon wool method and their purities are about 80%. (2) Both IL-2 and IFN-r mRNA expression and protein production could be detected in T lymphocytes induced by anti-CD3/CD28 Abs at 2 hr and 24 hr postactivtion, respectively. The cell proliferation in T lymphocytes could be detected at 72 hr postactivation. (4) Both IL-2 and IFN-r gene expression in T lymphocytes activated anti-CD3/CD28 Abs were regulated by ERK, P38, NF-kB, and NF-AT signaling pathways. (5) All K3, AC and DC reduced IL-2 and IFN-rmRNA transcripts and protein production and cell proliferation in T cells induced by anti-CD3 and anti-CD28 antibodies without cytotoxicity. (6) Both K3 and AC did not affect ERK and P38 activation in T lymphocytes stimulated with anti-CD3/CD28 Abs. DC decreased P38 phosphorylation in activated T lymphocytes. (7) The preliminary data from luciferase reporter assay showed that K3 and AC decreased NF-AT activation. (8) The results from electrophoresis mobility shift assay (EMSA) demonstrated that K3 impaired NF-AT and NF-kB DNA binding activities. We suggested that K3 suppressed IL-2 and IFN-r gene expression in T lymphocytes induced by anti-CD3/CD28 Abs related to reduction of NF-AT and NF-B activity. Furthermore, the detailed action mechanisms behind the differential effects of K3, AC, and DC on human T lymphocytes will be elucidated.
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