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1

Podgaec, Sérgio. "Padrões de resposta imune em pacientes com endometriose." Universidade de São Paulo, 2006. http://www.teses.usp.br/teses/disponiveis/5/5139/tde-31102006-105026/.

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Objetivo: O objetivo deste estudo foi analisar a relação e a predominância dos padrões de resposta imune Th1 e Th2 em pacientes com endometriose. Pacientes e Métodos: Entre Fevereiro de 2004 e Abril de 2005 foram avaliadas 98 pacientes divididas em dois grupos de acordo com a presença (Grupo A) ou ausência de endometriose (Grupo B), confirmada histologicamente. Foram coletados sangue periférico e fluido peritoneal de todas as pacientes para a dosagem de interleucinas (IL) 2, 4 e 10, fator de necrose tumoral-alfa (TNF-alfa) e interferon-gama (IFN-gama) por citometria de fluxo. Além da presença da endometriose, foram analisadas a fase do ciclo menstrual, o quadro clinico, o estadiamento, o local de acometimento e a classificação histológica da moléstia. Resultados: Observou-se elevação estatisticamente significante nas concentrações de IFN-gama (mediana de 1,5pg/ml no Grupo A e de 0,4pg/ml no Grupo B, p=0,03) e de IL-10 (mediana de 38,6pg/ml no Grupo A e de 15,7pg/ml no Grupo B, p=0,03) do fluido peritoneal das pacientes com endometriose em relação àquelas sem a doença. As pacientes com endometriose apresentaram alteração estatisticamente significativa na relação das concentrações de IL-4/IFN-gama (p<0,001), IL-4/IL-2 (p=0,006), IL-10/IFN-gama (p < 0,001) e IL-10/IL-2 (p<0,001) do fluido peritoneal, com concentrações mais elevadas da IL-4 e da IL-10, o que reflete o predomínio da resposta Th2 sobre a Th1. Conclusão: Os resultados obtidos permitem concluir que, neste estudo, observou-se elevação de citocinas relativas à resposta imune Th2, denotando haver um predomínio deste padrão de resposta em pacientes com endometriose.<br>Objective: The objective of this study was to analyze the relation and the predominance of the immune response patterns Th1 and Th2 in patients with endometriosis. Patients and Methods: Between February 2004 and April 2005, 98 patients were evaluated and divided into two groups, according to the presence (Group A) or absence of endometriosis (Group B), confirmed by histology. Peripheral blood and peritoneal fluid were collected from all patients to obtain the concentrations of interleukines (IL) 2, 4 and 10, tumor necrosis factor-alpha (TNF-alpha) and interferon-gamma (IFN-gamma) using flow cytometry. Besides the presence of endometriosis, we analyzed phase of menstrual cycle, clinical complaints, classification, site and histological differentiation of the disease. Results: We observed higher concentrations of IFN-gamma (median of 1.5pg/ml in Group A and 0.4pg/ml in Group B, p = 0.03) and IL-10 (median of 38.6pg/ml in Group A and 15.7pg/ml in Group B, p = 0.03) in peritoneal fluid of patients with endometriosis in relation to those without the disease. Patients with endometriosis presented a significant alteration in IL-4/IFN-gamma (p < 0.001), IL-4/IL-2 (p = 0.006), IL-10/IFN-gamma (p < 0.001) and IL-10/IL-2 (p<0.001) ratio concentrations of peritoneal fluid, with IL-4 and IL-10 predominance, reflecting a Th2 response predominance over the Th1. Conclusion: The results allow concluding that, in this study, it was observed a cytokine elevation related to Th2 immune response, indicating a predominance of this pattern of response in patients with endometriosis.
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Prendergast, Catriona Taguma. "Exploring the pathogenic potential of myelin-reactive Th1 and Th17 cells in central nervous system autoimmune disease." Thesis, University of Edinburgh, 2011. http://hdl.handle.net/1842/5285.

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The activation of naïve T cells results in their proliferation and differentiation into a particular T-helper (Th) phenotype, namely Th1, Th2 or Th17 cells. This thesis focuses on the role of pro-inflammatory Th1 and Th17 cells in the induction of autoimmune disease of the central nervous system (CNS), using murine experimental autoimmune encephalomyelitis (EAE) as the model. Classically, EAE has been considered to be a Th1-mediated disease. However, since the emergence of the Th17 cells, there has been a paradigm shift towards Th17 cells being the key pathogenic subset in autoimmune disease. This thesis established robust protocols for the differentiation of naïve T cells into myelin-reactive Th1 or Th17 cells, producing ‘clean’ populations devoid of any contaminating cells. Passive T cell-transfer experiments revealed that myelin-reactive Th1 cells could induce EAE, whereas Th17 cells could not. This lack of disease correlated with the inability of the Th17 cells to accumulate in the non-inflamed CNS. Myelin-reactive Th1 cells did have this capability and only once inflammation was established, could Th17 cells be identified in the CNS, potentially exacerbating the disease. After these differences were observed, the project investigated two main aims: 1) to identify differences in homing molecule expression on Th1 and Th17 cells which could explain the difference in their ability to home to the CNS, and to investigate the functional significance of such differences, by molecular blockade; 2) to investigate the requirements for three key cytokines in EAE pathogenesis in passive T cell transfer models, investigating IFN-γ,IL-17 and TNF-α. P-selectin glycoprotein ligand-1 appeared to be important for the initial entry of inflammatory T cells into the CNS. Th1 cells deficient in IFN-γ were capable of IFNinducing EAE. A proportion of the mice developed “atypical” clinical signs, which correlated with T cell infiltration predominantly of the brain, rather than the spinal cord. This atypical EAE may be IL-17 dependent. In conclusion, this thesis indicates the importance of not focusing all resources and therapeutic approaches on Th17- induced inflammation as Th17 cells may not play such a major role as previously thought.
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3

Costa, Fernando Augusto Miranda da. "Resposta imune in vitro aos antígenos de Papilomavírus Humano (HPV) em homens na cidade de São Paulo, Brasil." Universidade de São Paulo, 2013. http://www.teses.usp.br/teses/disponiveis/5/5133/tde-04022014-155625/.

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Introdução: O Papilomavírus Humano está muito bem associado com diversos tipos de cânceres humanos, como câncer anogenital e oral. Alguns estudos demonstram que o aparecimento de lesões e a progressão para o câncer estão relacionados ao tipo de resposta imune do hospedeiro. Deste modo, evidências indicam que a resposta imune do hospedeiro tem um papel muito importante para o curso da infecção pelo HPV. Objetivo: Avaliar a resposta imune específica in vitro ao Papilomavírus Humano (HPV) em homens com lesões causadas por HPV e sem lesão por HPV. Material e Métodos: Foram recrutados 31 pacientes e 11 voluntários, que formaram 4 grupos de estudo; sendo 12 pacientes no Grupo A (HIV +/ HPV +); 09 pacientes no Grupo B (HIV-/HPV+); 10 pacientes no Grupo C (HIV+/ HPV-); e 11 indivíduos saudáveis no Grupo D (HIV-/HPV-). Foram realizados ensaios de cultura celular para mensurar a resposta celular específica \"in vitro\" do tipo Th1/Th2/Th17 (INF-y, IL-2, TNFalfa, IL-4, IL-10 e IL-17) sob o estímulo da vacina quadrivalente do HPV (HPV 6, 11, 16 e 18) e à proteína E7 de HPV-16. Resultados: O grupo coinfectado (HIV +/ HPV+) apresentou níveis mais elevados de citocinas, principalmente do perfil Th2, comparando-se com os dados dos demais grupos de estudo. O grupo coinfectado apresentou níveis elevados de IL-6 e IL-10 (Perfil Th2) em relação ao grupo controle (HIV-/HPV-), com significância estatística (p < 0.0001 e p < 0.0001, respectivamente). Conclusão: Foi demonstrada uma elevada produção de citocinas no grupo HPV+/HIV+, sugerindo uma forte imunomodulação pela coinfecção HIV/HPV. Entretanto, novos estudos devem ser realizados para comprovar estes dados. Além de apresentar um perfil essencialmente Th2 do grupo coinfectado, principalmente pelos níveis elevados de IL-6 e IL-10 apresentados, sugerindo que estas duas citocinas possam servir como biomarcadores para persistência viral, uma vez que, os pacientes soropositivos para HIV apresentam maior persistência de HPV, e monitorar a progressão para lesões mais graves<br>Introduction: Human Papillomavirus is associated with different types of human cancers, such as anogenital and oral cancer. Some studies show that the appearance of lesions and progression to cancer are related to the type of host immune response. Thus, evidence indicates that the host immune response has a role key in the course of HPV infection. Objective: To evaluate the specific immune response in vitro to HPV in men with lesions caused by HPV and without injury caused by HPV. Methods: We recruited 31 patients and 11 volunteers, who formed four groups, with 12 patients in Group A (HIV+/HPV+); 09 patients in Group B (HIV-/HPV+); 10 patients in Group C (HIV+/HPV-) and 11 healthy subjects in Group D (HIV-/HPV-). Cells culture assay was performed to measure the specific immune response \"in vitro\" Th1/Th2/Th17 (IFN-y, IL-2, TNF-alfa, IL-4, IL-10 and IL-17) under the stimulation of quadrivalent HPV vaccine (HPV 6, 11, 16 and 18) and the E7 protein of HPV-16. Results: The coinfected group (HIV+/HPV+) had higher levels of cytokines, especially Th2 profile, compared with data from the other study groups. The coinfected group showed high levels of IL-6 and IL-10 (Th2 profile) compared to the control Group (HIV- /HPV-), with statistical significance (p < 0.0001 and p < 0.0001, respectively). Conclusion: This study demonstrated a high production of cytokines in the coinfected group, suggesting a strong immunomodulation by coinfection HIV/HPV. However, further studies should be conducted to confirm these data. In addition to presenting essentially a Th2 profile, especially by high levels of IL-6 and IL-10 presented, suggesting that these two cytokines may serve as biomarkers for viral persistence, since HIV seropositive patients have a higher persistence of HPV, and monitor the progression to more serious injuries
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4

Pereira, Leonardo Biscaro. "Avaliação do perfil de citocinas no tecido subcutâneo de camundongos na presença de cimento endodôntico." Universidade de São Paulo, 2013. http://www.teses.usp.br/teses/disponiveis/58/58135/tde-03102013-151254/.

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Avaliou-se a capacidade dos cimentos endodônticos: Sealapex®, Activ-GP® e AH-Plus® de alterarem o perfil das citocinas nas respostas Th1, Th2 e Th17, após a implantação destes em subcutâneo de camundongos. A quantificação das citocinas IL-2, IL-6, TNF-&alpha;, IFN-&gamma;, IL-4, IL-10 e IL-17 foi realizada in vivo, no tecido reacional circundante aos implantes, os quais foram confeccionados a partir de sondas nasogástricas estéreis e apirogênicas de cloreto de polivinila preenchidas com os cimentos, tendo um grupo controle com sondas vazias. Utilizou-se camundongos isogênicos da linhagem C57BL/6 machos de 6/8 semanas de vida sendo que cada um recebeu 2 implantes na região dorsal (lado direito e esquerdo). Após os períodos experimentais de 7, 21 e 63 dias, com os camundongos anestesiados, os implantes foram removidos juntamente com o tecido circundante, e os animais sacrificados em seguida por deslocamento cervical. As amostras de cada grupo foram divididas sendo: duas, contendo implante/tecido, processadas histotecnicamente e as demais com apenas tecido (sem implante) foram homogeneizadas e centrifugadas com solução formada por tampão RIPA e inibidor de protease. O sobrenadante, fruto deste processo, foi coletado e a dosagem das citocinas realizada através do kit CBA mouse-Th1/Th2/Th17 Cytokine Kit (BD Cytometric Bead Array, San Jose, CA, USA) em análise por citometria de fluxo. Os parâmetros avaliados foram a concentração da citocina em função do cimento testado em cada período experimental. Submeteu-se os resultados à análise estatística por meio do teste t com a correção de Welch\'s. Para todos os testes o nível de significância foi de 5%. Com relação à IL-2 houve diferenças estatísticas significantes entre os grupos Activ-GP® e AH-Plus® (p=0,0391). No período de 21 dias foram detectadas diferenças entre o grupo controle e AH-Plus® (p=0,0402) e entre o grupo Sealapex® e AH-Plus® (p=0,0244). O AH-Plus® induziou um maior aumento na IL-6, aos 7 dias em relação ao Activ-GP® (p=0,0286) e aos 21 dias entre o grupo controle (p=0.0402) e Activ-GP® (p=0.0244). Os níveis de TNF-&alpha; foram estatisticamente superiores após 7 dias quando comparou-se o grupo AH-Plus® com os demais. Observou-se que no grupo controle aos 7 e 21 dias ocorreram diferenças estatísticas em relação ao Sealapex® e AH-Plus® respectivamente quando avaliadas as concentrações de IFN-&gamma;. Houve também diferenças estatísticas entre o grupo controle e Sealapex® (p=0,0158) no período de 7 dias para a citocina IL-4. Os valores de IL-10 foram estatisticamente superiores para o grupo controle em relação ao Activ-GP® no período de 21 dias (p=0,0471). Com relação a IL-17 no período de 21 dias, observou-se os maiores valores para o grupo controle, seguido pelo Sealapex®, Activ-GP® e AH-Plus®. Foram detectadas diferenças entre os grupos controle e AH-Plus® (p=0,0121), controle e Activ-GP® (p=0,0262) e entre Sealapex® e Activ GP® (p=0,0314). Baseado nesses resultados podê-se concluir que: os cimentos endodônticos são capazes de modular as respostas Th1, Th2 e Th17 através da inibição ou estimulação da liberação das citocinas testadas. O cimento AH-Plus® promoveu as maiores diferenças no perfil de resposta Th1.<br>It was evaluated the capacity of the following endodontic sealers: Sealapex, Activ-GP and AH-Plus to modify the cytokine profile in Th1, Th2 and Th17 responses, after their implantation in the subcutaneous tissue of mice. Quantification of IL-2, IL-6, TNF-&alpha;, IFN-&gamma;, IL-4, IL-10 and IL-17 was performed in vivo, in the reactional tissue surrounding the implants, which were made from sterile nasogastric probes and apyrogenic of polyvinyl chloride filled with sealer, and a control group of empty probes. It was used isogenic mice of C57BL/6 lineage, 6/8 weeks old males, each of which received two implants in the dorsal region (left and right). After the experimental time of 7, 21 and 63 days, the mice were anesthetized and the implants were removed along with the surrounding tissue, the animals were then sacrificed by cervical dislocation. Samples from each group were divided as follows: two containing implant / tissue processed histologically and with only the remaining tissue (without implant) were mixed and centrifuged with a solution formed by RIPA buffer and protease inhibitors. The supernatant result of this process was collected and cytokine dosage accomplished by mouse-Th1/Th2/Th17 Cytokine CBA Kit Kit (BD cytometric Bead Array, San Jose, CA, USA) for flow cytometry analysis. The evaluated parameters were the cytokine concentration in function of sealer tested in each trial. The results were submitted to statistical analysis using the t test with Welch\'s correction. For all tests the significance level was 5%. With respect to IL-2 there were significant statistical differences between groups-Activ GP and AH-Plus (p=0.0391). In the period of 21 days differences were found between the control group and AH-Plus (p=0.0402) and between the group Sealapex and AH-Plus (p=0.0244). The AH-Plus induced a greater increase in IL-6, at 7 days compared to Activ-GP (p=0.0286) and at 21 days between the control group (p=0.0402) and Activ-GP (p=0.0244). The levels of TNF-&alpha; were significantly higher after 7 days when the AH-Plus group was compared with others. It was observed that in the control group at 7 and 21 days there were statistical differences in relation to Sealapex and AH-Plus respectively when evaluated concentrations of IFN-&gamma;. There were also significant differences between the control group and Sealapex (p=0.0158) within 7 days for the cytokine IL-4. The amounts of IL-10 were statistically higher in the control group compared to the Activ GP in a period of 21 days (p=0.0471). With respect to IL-17 in a period of 21 days, it was observed the highest values for the control group, followed by Sealapex, Activ-GP and AH-Plus. Differences were found between the control groups and AH-Plus (p=0.0121), control and Activ-GP (p=0.0262) and between Sealapex and Activ-GP (p=0.0314). Based on the presented results theendodontic sealers are able to promote changes in the response cytokine profile Th1, Th2 and Th17; Sealer AH-Plus produced the greatest changes, in the Th1 response profile.
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Morelli, Fernando Christiano Gabriel [UNESP]. "Quantificação de citocinas no conteúdo abomasal de bovinos de corte na presença ou ausência de ulceração gástrica." Universidade Estadual Paulista (UNESP), 2016. http://hdl.handle.net/11449/134249.

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Submitted by FERNANDO CHRISTIANO GABRIEL MORELLI null (fcgmorelli@yahoo.com.br) on 2016-02-12T17:49:35Z No. of bitstreams: 1 Fernando - Tese versão final Repositório UNESP.pdf: 1900802 bytes, checksum: a8c9044a1f5a46e203d3432398fc0a07 (MD5)<br>Approved for entry into archive by Sandra Manzano de Almeida (smanzano@marilia.unesp.br) on 2016-02-15T11:32:07Z (GMT) No. of bitstreams: 1 morelli_fcg_dr_araca.pdf: 1900802 bytes, checksum: a8c9044a1f5a46e203d3432398fc0a07 (MD5)<br>Made available in DSpace on 2016-02-15T11:32:07Z (GMT). No. of bitstreams: 1 morelli_fcg_dr_araca.pdf: 1900802 bytes, checksum: a8c9044a1f5a46e203d3432398fc0a07 (MD5) Previous issue date: 2016-02-01<br>Erosões e úlceras são achados comuns no abomaso e causam preocupação econômica nos mais variados sistemas de produção de gado. Muitos fatores podem predispor ao aparecimento de úlceras e acúmulo de gases no abomaso, incluindo alimentos grosseiros, estresse ambiental, deficiências de vitaminas e minerais e infecções bacterianas. Essas úlceras podem ser subclínicas, sendo descobertas nas necropsias ou após o abate do animal, ou levarem à redução da motilidade do órgão, prejudicando o fluxo do seu conteúdo e causando transtornos digestivos graves e até ao aparecimento de síndromes semelhantes à indigestão vagal. Existem informações a respeito da resposta do sistema imune na maior parte das mucosas do trato gastrintestinal de não-ruminantes e ruminantes, porém são raras a respeito do abomaso. Os objetivos desse estudo foram detectar os níveis de citocinas (IL-17A, IFN-γ, TNF-α, IL-10, IL-6, IL-4, IL-2) no conteúdo abomasal em bovinos de corte, determinar o perfil Th1 ou Th2 dessas citocinas em animais com úlceras de grau 1 e 2 na região cárdica abomasal e comparar esses valores com os níveis de citocinas de animais sem úlceras (controle), em amostras colhidas em abatedouro, para auxiliar na compreensão da fisiopatologia do processo inflamatório local. A avaliação macroscópica e a classificação das úlceras foi realizada por meio de exames visual e histológico em amostras de tecidos da parede da região cárdica abomasal ulcerada. Os níveis de citocinas produzidas do líquido abomasal dos animais com ou sem úlceras foram avaliados por citometria de fluxo (método Cytometric Bead Array). As citocinas citadas foram detectadas no líquido do abomaso dos bovinos. Não houve diferença na liberação das citocinas entre os grupos com úlceras e o grupo sem úlcera, indicando um equilíbrio entre perfis Th1 e Th2 da resposta inflamatória.<br>Erosions and ulcers are common findings in the abomasum and cause economic concern in several livestock production systems. Many factors may predispose to ulcers and bloat in the abomasum, including roughage, environmental stress, deficiencies of vitamins and minerals and bacterial infections. These ulcers may be subclinical and are found during necropsy or after slaughter, or lead to reduction of abomasal motility, hindering the flow of your content and causing serious digestive disorders and even the appearance of syndromes similar to vagal indigestion. There are some studies evaluating the immune system response in most of the mucous membranes of the gastrointestinal tract of non-ruminants and ruminants, but rarely related to the abomasum. The aims of this study were to investigate the levels of cytokines (IL-17A, IFN-γ, TNF-α, IL-10, IL-6, IL-4, IL-2) in the abomasal fluid of beef cattle, to determine the Th1 or Th2 profile of these cytokines in animals with types 1 or 2 ulcers located in the abomasal cardic region and to compare these levels with those of animals without ulcers (controls), in samples collected in an abbatoir, to help to the understand the pathophysiology of the local inflammatory process. Ulcers from the abomasal cardic region were macroscopicaly evaluated, then classified by histology. Cytokine levels in the abomasal fluid from animals with or without ulcers were evaluated by flow cytometry (Cytometric Bead Array). Cytokines were detected in the abomasum fluid of cattle. There was no difference in the release of cytokines between groups, indicating a balance between Th1 and Th2 profiles of the inflammatory response.
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Morelli, Fernando Christiano Gabriel. "Quantificação de citocinas no conteúdo abomasal de bovinos de corte na presença ou ausência de ulceração gástrica /." Araçatuba, 2016. http://hdl.handle.net/11449/134249.

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Orientador: Juliana Regina Peiró<br>Banca: Lina Maria Wehrle Gomide<br>Banca:Fernanda Bovino<br>Banca: José Paes de Oliveira Filho<br>Banca:Glenda Nicioli da Silva<br>Resumo: Erosões e úlceras são achados comuns no abomaso e causam preocupação econômica nos mais variados sistemas de produção de gado. Muitos fatores podem predispor ao aparecimento de úlceras e acúmulo de gases no abomaso, incluindo alimentos grosseiros, estresse ambiental, deficiências de vitaminas e minerais e infecções bacterianas. Essas úlceras podem ser subclínicas, sendo descobertas nas necropsias ou após o abate do animal, ou levarem à redução da motilidade do órgão, prejudicando o fluxo do seu conteúdo e causando transtornos digestivos graves e até ao aparecimento de síndromes semelhantes à indigestão vagal. Existem informações a respeito da resposta do sistema imune na maior parte das mucosas do trato gastrintestinal de não-ruminantes e ruminantes, porém são raras a respeito do abomaso. Os objetivos desse estudo foram detectar os níveis de citocinas (IL-17A, IFN-γ, TNF-α, IL-10, IL-6, IL-4, IL-2) no conteúdo abomasal em bovinos de corte, determinar o perfil Th1 ou Th2 dessas citocinas em animais com úlceras de grau 1 e 2 na região cárdica abomasal e comparar esses valores com os níveis de citocinas de animais sem úlceras (controle), em amostras colhidas em abatedouro, para auxiliar na compreensão da fisiopatologia do processo inflamatório local. A avaliação macroscópica e a classificação das úlceras foi realizada por meio de exames visual e histológico em amostras de tecidos da parede da região cárdica abomasal ulcerada. Os níveis de citocinas produzidas do líquido abomasal... (Resumo completo, clicar acesso eletrônico abaixo)<br>Abstract: Erosions and ulcers are common findings in the abomasum and cause economic concern in several livestock production systems. Many factors may predispose to ulcers and bloat in the abomasum, including roughage, environmental stress, deficiencies of vitamins and minerals and bacterial infections. These ulcers may be subclinical and are found during necropsy or after slaughter, or lead to reduction of abomasal motility, hindering the flow of your content and causing serious digestive disorders and even the appearance of syndromes similar to vagal indigestion. There are some studies evaluating the immune system response in most of the mucous membranes of the gastrointestinal tract of non-ruminants and ruminants, but rarely related to the abomasum. The aims of this study were to investigate the levels of cytokines (IL-17A, IFN-γ, TNF-α, IL-10, IL-6, IL-4, IL-2) in the abomasal fluid of beef cattle, to determine the Th1 or Th2 profile of these cytokines in animals with types 1 or 2 ulcers located in the abomasal cardic region and to compare these levels with those of animals without ulcers (controls), in samples collected in an abbatoir, to help to the understand the pathophysiology of the local inflammatory process. Ulcers from the abomasal cardic region were macroscopicaly evaluated, then classified by histology. Cytokine levels in the abomasal fluid from animals with or without ulcers were evaluated by flow cytometry (Cytometric Bead Array). Cytokines were detected in the abomasu... (Complete abstract click electronic access below)<br>Doutor
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Ganakammal, Satishkumar Ranganathan. "CIS REGULATORY MODULE DISCOVERY IN TH1 CELL DEVELOPMENT." Thesis, Proceeding ISB '10 Proceedings of the International Symposium on Biocomputing ACM New York, NY, USA ©2010 table of contents ISBN: 978-1-60558-722-6 doi>10.1145/1722024.1722039, 2010. http://hdl.handle.net/1805/2678.

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Indiana University-Purdue University Indianapolis (IUPUI)<br>Immune response enables the body to resist foreign invasions. The Inflammatory response is an important aspect in the immune response which is articulated by elements such as cytokines, APC, T-cell and B-cell, effector cell or natural killer. Of these elements, T-cells especially T-helper cells; a sub class of T-cells plays a pivotal role in stimulating the immune response by participating in various biological reactions such as, the transcription regulatory network. Transcriptional regulatory mechanisms are mediated by a set of transcription factors (TFs), that bind to a specific region (motifs or transcription factor binding sites, TFBS), on the target gene(s) controlling the expression of genes that are involved in T-helper cell mediated immune response. Eukaryotic regulatory motifs, referred to as cis regulatory modules (CRMs) or cistrome, co-occur with the regulated gene’s transcription start site (TSS) thus, providing all the essential components for building the transcriptional regulatory networks that depends on the relevant TF-TFBS interactions. Here, we study IL-12 stimulated transcriptional regulators in STAT4 mediated T helper 1 (Th1) cell development by focusing on the identification of TFBS and CRMs using a set of Stat4 ChIP-on-chip target genes. A region containing 2000 bases of Mus musculus sequences with the Stat4 binding site, derived from the ChIP-on-chip data, has been characterized for enrichment of other motifs and, thus CRMs. Our experiments identify some potential motifs, (such as NF-κB and PPARγ/RXR) being enriched in the Stat4 binding sequences compared to neighboring background sequences. Furthermore, these predicted CRMs were observed to be associated with biologically relevant target genes in the ChIP-on-chip data set by meaningful gene ontology annotations. These analyses will enable us to comprehend the complicated transcription regulatory network and at the same time categorically analyze the IL-12 stimulated Stat4 mediated Th1 cell differentiation.
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Rehorova, Hradilkova Kristyna. "Role of Twist1 in metabolism of repeatedly stimulated Th1 cells." Doctoral thesis, Humboldt-Universität zu Berlin, 2019. http://dx.doi.org/10.18452/20584.

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Es stellt sich die Frage, wie diese Zellen im entzündeten Gewebe überleben können und wie sie ihren Stoffwechsel an die dortigen Bedingungen anpassen. Diese Arbeit beschreibt am Beispiel der Juvenilen Idiopathischen Arthritis (JIA) die Analyse des Stoffwechsels von CD4+ T Lymphozyten, die chronische Entzündungen antreiben undim entzündeten Gewebe lange Zeit persistieren. Pathogene CD4+ CD45RO+ PD1+ CXCR5-T Zellen wurden hierfür aus Synovialflüssigkeit von Patienten mit JIA isoliert und gezeigt, dass auch bei diesen Zellen der Stoffwechsel auf Fettsäureoxidation beruht. Wurde die Fettsäureoxidation durch Etomoxir blockiert, starben die Zellen. Die Störung des Stoffwechsels dieser Zellen könnte somit eine Option für einen neuen Therapieansatzdarstellen. Zusätzlich war die Expression des Transkriptionsfaktors Twist 1 in diesen CD4+CD45RO+ PD1+ CXCR5- T Zellen hochreguliert. Twist 1 ist ein Marker für T Lymphozyten, die in entzündetem Gewebe von Patienten mit chronisch-entzündlichen Erkrankungen der Gelenke oder des Darmes persistieren. Untersuchung in vitro ergaben außerdem, dass Twist 1 spezifisch von Th1 Lymphozyten exprimiert wird, die mehrfach restimuliert wurden. Dieser Transkriptionsfaktor wirkt einerseits der Gewebszerstörung, die von T Zellen verursacht wird, entgegen, und unterstützt anderseits die Persistenz der Zellen im Gewebe durch die Induktion der microRNA148a, die die Expression des pro-apoptotischen Proteins Bim reguliert. In dieser Arbeit zeigen wir dessen Einfluss auf die Regulation des Metabolismus von CD4+ T Lymphozyten bei chronischen Entzündungen. Dabei wird die Glycolyse verringert und vermehrt Fettsäuren synthetisiert, um die Zellen vor reaktiven oxidierenden Spezies (ROS) zu schützen. Zusätzlich konnten wir nachweisen, dass mehrfach re-stimulierte, Twist-defizienteTh1 Zellen unfähig sind, durch Fettsäureoxydation zu überleben, sondern den Stoffwechsel auf Lipid- Peroxidierung umstellen<br>How do CD4+ T cells adapt their metabolism for survival in the inflamed tissue? This thesis describes analysis of the metabolism of CD4 T lymphocytes driving chronic inflammation and persisting at the site of inflammation, exemplified by cells that reside in the inflamed tissue of patients with the rheumatic disease juvenile idiopathic arthritis. To specifically take aim at the CD4+ T lymphocytes persisting at the site of inflammation, it is important to determine how these cells adapt their metabolism. We show that pathogenic CD4+ CD45RO+ PD1+ CXCR5- T cells that were isolated from the synovial fluid of patients with juvenile idiopathic arthritis are dependent on a fatty acid oxidation for survival ex vivo. Their survival can be blocked by blocking FAO with Etomoxir, pointing to the option of targeting such cells by metabolic interference. Furthermore, CD4+ CD45RO+ PD1+ CXCR5- T cells had upregulated expression of Twist1, a hallmark transcription factor of T lymphocytes persisting in the inflamed tissues of patients with chronic-inflammatory diseases of joints or the gut. Expression of Twist1 is specific for Th1 lymphocytes which have repeatedly been re-stimulated in vitro, or isolated from inflamed. This transcription factor dampens immunopathology caused by the T cells and supports their persistence, by inducing microRNA148a, which regulates expression of the proapoptotic protein Bim. This thesis shows, through conditional genetic inactivation of Twist1 in CD4+ T lymphocytes, that Twist1 regulates the metabolism ofCD4 T lymphocytes of chronic inflammation, by downregulating glycolysis, promoting fatty acid synthesis and protecting the cells from ROS. Additionally, we show that Twist1 deficient repeatedly reactivated murine Th1 cells are unable to survive on fatty acid oxidation and have increased levels of lipid peroxidation.
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Esfandiari, Ehsanollah. "Role of Th1 and Th2 cytokines in the pathogenesis of systemic autoimmune diseases." Thesis, University of Glasgow, 2001. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.366255.

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10

Yamori, Masashi. "Antigenic activation of Th1 cells in the gastric mucosa enhance dysregulated apoptosis and turnover of the epithelial cells." Kyoto University, 2004. http://hdl.handle.net/2433/145273.

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Hardaway, John C. Zaghouani Habib. "Examination of neonatal immunity in IL-13 receptor alpha 1 deficient mice." Diss., Columbia, Mo. : University of Missouri-Columbia, 2009. http://hdl.handle.net/10355/6977.

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The entire dissertation/thesis text is included in the research.pdf file; the official abstract appears in the short.pdf file (which also appears in the research.pdf); a non-technical general description, or public abstract, appears in the public.pdf file. Title from PDF of title page (University of Missouri--Columbia, viewed on January 5, 2010). Vita. Thesis advisor: Habib Zaghouani. Includes bibliographical references.
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Jonsson, Yvonne. "Cytokines and immune balance in preeclampsia : a survey of some immunological variables and methods in the study of preeclampsia." Doctoral thesis, Linköping : Linköpings universitet, 2005. http://www.bibl.liu.se/liupubl/disp/disp2005/med924s.pdf.

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13

Zhang, W., X. Tian, F. Mumtahana, et al. "The existence of Th22, pure Th17 and Th1 cells in CIN and Cervical Cancer along with their frequency variation in different stages of cervical cancer." BioMed Central Ltd, 2015. http://hdl.handle.net/10150/610273.

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BACKGROUND: Recently, it is found that T-helper (Th) 22 cells are involved in different types of autoimmune and tumor diseases. But, till now, no study has been carried out to understand the involvement of these cells in cervical cancer (CC). METHODS: Flow cytometry was used to determine the expression of interferon gamma (IFN-gamma), Interleukin-22 (IL-22), IL-17 in the peripheral blood of healthy controls (HC), CIN and cervical cancer patients. From peripheral blood mononuclear cells (PBMCs), mRNA expression levels of Aryl hydrocarbon receptor (AHR), RAR-related orphan receptor C (RORC), TNF-alpha and IL-6 were respectively determined. Using the method of ELISA, plasma concentrations of IL-22, IL-17 and TNF-alpha were examined. RESULTS: Th22 and Th17 cells were elevated in CC and CIN patients. Th1 cells and the plasma concentrations of IL-22 in CC patients were significantly increased compared with HC. In CC patients, an increased prevalence of Th22 cells was associated with lymph node metastases. There was a positive correlation between Th22 and Th17 cells, but an approximately negative correlation between Th22 and Th1 cells in CC patients. The mRNA expression of RORC, TNF-alpha and IL-6 was significantly high in CC patients. CONCLUSIONS: Our results indicate that there is a higher circulatory frequency of Th22, Th17 and Th1 cells in CC which may conjointly participate in the pathogenesis and growth of CC.
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Szymczak, Wendy A. "The Role Of Chemokines and Dendritic Cells In Regulation of IL-4 and Fungal Immunity." University of Cincinnati / OhioLINK, 2010. http://rave.ohiolink.edu/etdc/view?acc_num=ucin1266607502.

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15

Cantor, Joseph M. "Effector function of pathogenic CD4 TH1 T cells in autoimmune diabetes /." Connect to full text via ProQuest. IP filtered, 2005.

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Thesis (Ph.D. in Immunology) -- University of Colorado, 2005.<br>Typescript. Includes bibliographical references (leaves 180-202). Free to UCDHSC affiliates. Online version available via ProQuest Digital Dissertations;
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Lee, Hyun-Hee. "Immunity in the newborn control by IL-13 receptor and dendritic cells /." Diss., Columbia, Mo. : University of Missouri-Columbia, 2007. http://hdl.handle.net/10355/5939.

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Thesis (Ph. D.)--University of Missouri-Columbia, 2007.<br>"May 2007" The entire dissertation/thesis text is included in the research.pdf file; the official abstract appears in the short.pdf file (which also appears in the research.pdf); a non-technical general description, or public abstract, appears in the public.pdf file. Vita. Includes bibliographical references.
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17

Consentius, Christine. "Inhibition of the crosstalk between dendritic, natural killer and T cells by mesenchymal stromal/stem cells." Doctoral thesis, Humboldt-Universität zu Berlin, Lebenswissenschaftliche Fakultät, 2016. http://dx.doi.org/10.18452/17694.

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Mesenchymale Stromazellen (MSC) unterstützen die endogene Geweberegeneration und sind kaum immunogen. Die Mechanismen der Immunmodulation sind kaum bekannt. Diese Arbeit untersucht, ob MSC in die Interaktion von Dendritischen Zellen (DC), Natürlichen Killer (NK) und T Zellen eingreifen, indem sie die DC-Reifung beeinflussen. Das Netzwerk ist wichtig für die Differenzierung naïver T Zellen zu Typ 1 T Helferzellen (Th1). Abhängig vom DC-Subtyp und dem Zeitpunkt des Aufeinandertreffens, beeinflussten Knochenmark-MSC (BM-MSC) die in vitro DC-Reifung verschieden. Sie inhibierten die Differenzierung, aber nicht die Reifung humaner von Monozyten-abgeleiteter DC (moDC). BM MSC hatten keinen klaren Einfluss auf die Reifung plasmazytoider DC (pDC), während sie in aktivierten CD1c+ myeloiden DC (mDC) einen tolerogenen Phänotyp induzierten, charakterisiert durch eine geringere CCR7-abhängige Migration und ein tolerogenes Zytokinprofil. Daraus resultierend, wiesen BM-MSC-geprägte mDC aufgrund der veränderten IL 12/IL 10 Sekretion eine geringere Fähigkeit zur Stimulation der IFNγ Produktion in NK Zellen auf und induzierten weniger Th1 Differenzierung naïver T Zellen. Placenta-derived mesenchymal-like adherent stromal cells (PLX PAD) erzielten ähnliche Ergebnisse. Es konnte keine Alloimmunogenität in Patienten mit kritischer Ischämie der Extremitäten (CLI), die im Rahmen einer Phase I klinischen Studie allogene PLX PAD erhalten hatten, nachgewiesen werden. Keiner der Patienten entwickelte eine signifikante Gedächtnis T Zellantwort spezifisch für das Zellprodukt, was durch unsere in vitro Beobachtungen erklärbar sein könnte. Es ist schwierig MSC im Gewebe nachzuweisen, da Markerkombinationen notwendig sind. CD73+CD90+CD105+CD45-CD34-CD14-CD19- MSC konnten mithilfe einer neuen Multiplex-Immunhistologie-Technik (Chipzytometrie) in humanen Plazentaschnitten detektiert werden. Für die Zukunft könnte damit die Interaktion injizierter MSC mit Immunzellen in Biopsien untersucht werden.<br>Mesenchymal stromal cells (MSC) support endogenous tissue regeneration and seem to be low immunogenic, allowing application across MHC barriers. But little is known about the mechanisms for their immunomodulation. Hence, the main goal of this study was to understand if MSC interfere with the crosstalk between dendritic cells (DC), natural killer (NK) and T cells by influencing DC maturation. This network is important for efficient priming of naïve T cells into type 1 helper T cells (Th1). Bone marrow-derived MSC (BM-MSC) had diverse effects on DC maturation in vitro, depending on the DC subset and the time of interaction. BM MSC inhibited differentiation but not maturation of monocyte-derived DC (moDC). They did not have a clear effect on maturation of plasmacytoid DC (pDC), whereas they induced a tolerogenic phenotype in activated CD1c+ myeloid DC (mDC), characterized by an impaired CCR7-dependent migration and a tolerogenic cytokine profile. Consequently, BM-MSC-licensed mDC displayed a reduced ability to induce IFNγ production in NK cells due to their altered IL 12/IL 10 secretion. BM MSC-licensed mDC also induced less efficiently Th1 lineage commitment of naïve T cells. Similar results were observed with placenta-derived mesenchymal-like adherent stromal cells (PLX PAD). Samples from critical limb ischemia (CLI) patients treated with MHC-unmatched PLX-PAD within a phase I clinical trial were analysed for alloimmunogenicity. None of the patients developed a significant memory T cell response specific to the allogeneic cells, which might be explainable by our in vitro observations. MSC are difficult to detect in tissues because a set of lineage markers is needed. Here, CD73+CD90+CD105+CD45-CD34-CD14-CD19- MSC could be identified in human placenta cryosections using a novel multiplex-immunohistology technique (chipcytometry), offering the possibility to investigate the crosstalk between injected MSC and attracted immune cells in patient biopsies in the future.
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Nowakowska, Dominika Joanna. "Phenotype and function of regulatory T cells in Th1- and Th2-mediated inflammatory diseases." Thesis, University of Edinburgh, 2013. http://hdl.handle.net/1842/11779.

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Regulatory T cells (Treg) are critical to the maintenance of immune tolerance, partly by controlling the unwanted activation of effector T cells (Teff) and thereby enhancing the resolution of autoimmune and allergic inflammation. Recent data suggest that Treg can specialize to better control different types of inflammation by using transcriptional machinery which controls differentiation and function of Teff. This thesis addresses questions related to the efficacious use of Treg, notably their ability to adopt distinct phenotypic profiles under different inflammatory contexts and their need to recognize antigen in the inflamed organ. Two differentially mediated mouse disease models were used in this project, namely Th1/Th17-mediated experimental autoimmune encephalomyelitis (EAE) as a model of multiple sclerosis and Th2-mediated allergic airways inflammation (AAI) as a model of asthma. A new model of rMOG-induced AAI was developed to specifically answer the questions on the importance of cell phenotype versus antigen-reactivity for the effective Treg-mediated suppression. It was demonstrated that Treg from the inflamed CNS in EAE had an upregulated expression of Th1 master regulator T-bet and Th1-associated chemokine receptor CXCR3, whereas Treg derived from the inflamed lung in AAI had an increased expression of Th2 master regulator GATA-3, lacked expression of T-bet and displayed decreased levels of CXCR3. This specialized and activated phenotype was restricted to tissue-derived Treg. The importance of appropriate Treg phenotype for effective suppression was suggested by the observed inability of CNS-derived Treg to inhibit AAI. A different Treg subset, TGF-β-induced Treg (iTreg), was shown to express high levels of T-bet and CXCR3, but not GATA-3 upon induction in vitro. iTreg effectively suppressed both Th1 and Th2 types of inflammation and the antigenreactivity was key to this. This thesis demonstrates that Treg are capable of acquiring a distinct phenotype corresponding with a CD4+ T cell response driving inflammatory disease and identifies antigen-reactivity as key to the efficacious suppression of inflammation. It also highlights substantial phenotypic differences between iTreg and naturally-occurring Treg which could be associated with different modes of suppression.
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Huang, Emily Chi Ping. "Effect of Pharmacological Calcium Mobilization as a Co-signal Regulating IL-12 Production by Murine Dendritic Cells." Kent State University / OhioLINK, 2014. http://rave.ohiolink.edu/etdc/view?acc_num=kent1397923386.

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Huss, David J. "Effector Th1 cells demonstrate self-regulation in a mouse model of Multiple Sclerosis." The Ohio State University, 2011. http://rave.ohiolink.edu/etdc/view?acc_num=osu1305118647.

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VENZIN, VALENTINA. "Th1-LIKE HBV-SPECIFIC CD4+T CELLS ARE ABLE TO REVERT THE CD8+T CELL DYSFUNCTION INDUCED BY HEPATOCELLULAR PRIMING." Doctoral thesis, Università Vita-Salute San Raffaele, 2023. https://hdl.handle.net/20.500.11768/137016.

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About 260 million people are chronically infected with hepatitis B virus (HBV), resulting in >700,000 deaths per year from cirrhosis and hepatocellular carcinoma. Despite the availability of prophylactic vaccination, therapeutic approaches for persistent infection are still limited. The immune mechanisms underlying Hepatitis B Virus (HBV) pathogenesis are still not delineated, and while the function and dysfunction of CD8+T cells has been deeply investigated, the role of HBV-specific (HBV-sp) CD4+T cells has been neglected. With the aim of studying the role of CD4+T cells in the context of HBV pathogenesis, we have generated and tested an HBV-sp CD4+TCR transgenic mouse model (Env126), in which all CD4+T cells recognize an MHC class II-restricted epitope of the HBV envelope protein. Here, we used a mouse model of HBV pathogenesis, where adoptively transferred HBV-sp naive CD8+T cells recognizing hepatocellular antigens are driven into a state of immune dysfunction. We found that pre-activated Th1-like Env126 CD4+TE cells can revert CD8+T cells dysfunctionality after adoptive co-transfer in HBV-replicating mice. With the help of Env126 CD4+TE cells, HBV-sp CD8+T cells produce higher levels of IFNɣ, TNF⍺ and GrzmB, increase their proliferation capacity and display higher expression levels of activation markers as well as reduction in co-inhibitory molecules. Moreover, we observed that Kupffer cells can ameliorate their cross-presenting capacity and upregulate MHC-I machinery after adoptive transfer of Env126 CD4+TE cells in HBV-Tg mice. Indeed, we confirmed CD4+-CD8+T cell cooperation is abolished if APCs are not able to interact with Env126 CD4+TE cells in HBV-Tg mice. These preliminary results show that HBV-sp CD4+T cells might have a critical role in defining the course of HBV pathogenesis. As main cooperators of CD8+T cells antiviral immunity, HBV-sp CD4+T cells spatiotemporal dynamics must be elucidated, helping the design of novel immunotherapeutic strategies aimed at treating HBV infection and its life-threatening complications.<br>Circa 260 milioni di persone hanno attualmente un’infezione cronica da virus dell’epatite B, portando il numero di morti all’anno causate da carcinoma epatico a 700000. Nonostante sia disponibile una vaccinazione preventiva, gli approcci terapeutici per curare l’infezione persistente da HBV sono ancora limitati. I meccanismi che determinano la patogenesi da HBV non sono ancora del tutto chiariti e, mentre la funzionalità e disfunzionalità delle cellule T CD8 è stata approfonditamente studiata, il ruolo delle cellule T CD4 specifiche per HBV è stato trascurato. Con lo scopo di studiare il ruolo delle cellule T CD4 nel contento della patogenesi di HBV, abbiamo generato e testato un modello murino transgenico (Env126) in cui tutte le cellule T CD4 riconoscono un peptide specifico della proteina di superficie di HBV. In questo studio abbiamo utilizzato un modello murino di patogenesi di epatite B, dove, dopo essere state iniettate, le cellule T CD8 specifiche per HBV diventano disfunzionali in seguito a priming epatocellulare. Abbiamo osservato che, in questo contesto, il trasferimento contemporaneo di cellule T CD4 effettrici con un fenotipo T helper 1 è in grado di revertire la disfunzionalità delle cellule T CD8. Grazie all’aiuto fornito dalle cellule T CD4 Env126, le cellule T CD8 specifiche per HBV sono in grado di produrre livelli maggiori di IFNg, TNFa e GrzmB, sono in grado di proliferare di più e ridurre l’espressione di molecole inibitorie sulla loro superficie. Abbiamo inoltre osservato che le cellule Kupffer nel fegato, sono in grado di migliorare la loro capacità di cross-presentazione antigienica dopo il trasferimento delle cellule T CD4 Env126 effettrici. Infatti, abbiamo inoltre confermato che la cooperazione CD4-CD8 nel nostro contesto non è più presente se le cellule presentanti l’antigene consono più in grado di interagire con le cellule T CD4 Env126 effettrici. Questi risultati preliminari mostrano in conclusione che le cellule T CD4 potrebbe avere un ruolo importante nel definire il corso della patogenesi di HBV. Essendo le cellule principali coordinatrici della risposta antivirale CD8 specifica, la dinamica della risposta T CD4 andrebbe approfondita, con lo scopo ultimo di aiutare nella creazione di nuove strategie terapeutiche in grado di trattare l’infezione da HBV e le sue più gravi complicazioni.
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Saul, Alison Nicole. "Psycho-physiological stress and its effects on ultraviolet light induced inflammation, DNA damage, and skin carcinogenesis." Columbus, Ohio : Ohio State University, 2007. http://rave.ohiolink.edu/etdc/view?acc%5Fnum=osu1172850801.

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Dubois, Natasha. "Caractérisation de la réponse immune induite par un adjuvant comprenant un agoniste du TLR4 dans des modèles murins." Thesis, Université Paris-Saclay (ComUE), 2016. http://www.theses.fr/2016SACLS131/document.

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En 2014 la Tuberculose (TB) à dépassé le VIH comme la principale cause de décès par maladie infectieuse dans le monde soulignant le besoin urgent de développer un vaccin plus efficace contre cette maladie. Le candidat vaccin contre la TB, ID93/GLA-SE, dévéloppé à l’Infectious Disease Research Institute (IDRI), est aujourd’hui en essai clinique de phase IIa et a montré des résultats pré-cliniques et cliniques promettants. Dans de modèle murin de TB, ce vaccin induit une forte réponse TH1, considérée comme centrale dans la protection contre la TB, et la production d’IgG2 par les lymphocytes B. Néanmoins, les mécanismes d’action de GLA-SE sont encore peu connus.L’objectif principal de cette thèse est donc d’élucider les méchanismes clés qui relient les réponses innées et adaptatives induites par cet adjuvant dans le modèle murin. Un objectif secondaire est d’établir un modèle murin de rechute de TB après traitement et d’évaluer l’utilisation d’ID93/GLA-SE en tant que vaccin immuno-thérapeutique et sa capacité à réduire les taux de rechute dans ce modèle. L‘ensemble de ce travail nous a permis de mieux comprendre les mécanismes impliqués dans la réponse immunitaire adaptative induite par GLA- SE et de montrer la capacité de ID93/GLA- SE a être utilisé comme un vaccin thérapeutique contre la tuberculose dans le but de réduire les taux de rechute post-thérapeutiques<br>In 2014 tuberculosis (TB) surpassed HIV as the leading cause of death by an infectious disease worldwide emphasizing the urgent need to develop a more effective vaccine against this airborne disease. The Infectious Disease Research Institute (IDRI) TB candidate vaccine ID93/GLA-SE is currently undergoing a Phase IIa clinical trial and has shown promising preclinical and clinical results. In murine models of TB this vaccine drives a strong CD4 TH1 response, which is thought to be important for protection against TB, and an IgG2c skewed B cell response. However, little is known about the cellular and molecular events that drive GLA-SE adjuvanticity.To that end, the main objective of my thesis was to elucidate the key mechanisms that connect innate and adaptive immune responses elicited by this adjuvant in the murine model. A secondary objective was to evaluate the possibility of using ID93/GLA-SE as adjunct therapy to existing antibiotic treatments to reduce relapse rates after TB treatment.Collectively the results obtained during this research project and thesis broaden our knowledge and our current understanding of the mechanisms involved in the adaptive immune response induced by GLA-SE and show the capacity of ID93/GLA-SE to be used as a therapeutic vaccine against TB to reduce post-therapeutic relapse rates
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Silveira, Denise Sayuri Calheiros da. "Papel funcional dos leucotrienos na resposta imunológica ao melanoma B16-F0 experimental em camundongos." Universidade de São Paulo, 2012. http://www.teses.usp.br/teses/disponiveis/60/60135/tde-28062012-144450/.

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No presente trabalho investigamos a relevância dos mediadores lipídicos (Leucotrienos) gerados pela enzima 5-Lipoxigenase (5-LO) na susceptibilidade ou resistência de camundongos ao Melanoma experimental com células tumorais B16-F0, utilizando como modelo camundongos produtores de leucotrienos (129_WT) e camundongos geneticamente deficientes \"knockout\" de 5-LO (129_5-LO KO). Primeiramente, verificamos que leucócitos peritoneais provenientes de animais WT implantados com melanoma B16-F0, apresentam aumento da expressão do gene para 5-LO (Alox5). Nossos resultados mostram que animais 5-LO KO, deficientes de 5-LO são mais eficientes no controle da progressão do tumor e apresentam significativo aumento na sobrevivência, quando comparados a animais WT, produtores de 5-LO. A nossa análise do perfil imunológico em células esplênicas indicam que a maior eficiência dos camundongos 5-LO KO no controle do crescimento de células tumorais B16-F0 estariam associados à presença numérica aumentada de neutrófilos (Gr-1+), células apresentadoras de antígeno (I-Ab+) majoritariamente CD19+CD80+ e esplenócitos capacitados para produção de altos níveis de citocinas pró-inflamatórias/efetoras como a IL-6, TNF?, IFN-? e baixos níveis de citocinas regulatórias como IL-10, 15 dias pós-implantação do tumor; a rápida geração da resposta imune polarizada para produção elevada de citocinas Th1 (IFN-?), mas não, citocinas Th2 (IL-10) e presença de maiores números de linfócitos T CD4+ e CD8+ efetoras, expressando o fenótipo CD44high ou CD44highCD62Llow. Ainda, verificamos que a deficiência genética da 5-LO ou a inibição da 5-LO pelo MK886 em células LAK, aumenta significativamente sua atividade citotóxica em células do melanoma B16-F0. Nossos resultados em conjunto, indicam que leucotrienos gerados pela enzima 5-LO, modulam negativamente a geração de resposta imune protetora em camundongos para o Melanoma B16-F0.<br>In the present work we examine the contribution of 5-lipoxigenase-derived lipid mediators during experimental melanoma (B16-F0) in 5-LO gene knockout (KO) mice and wild-type (WT) mice. The 5-LO KO mice presented delayed tumor growth, lesser tumor volume and delayed mortality. The greater resistance of 5-LO KO mice correlated with the following: High splenic Gr-1+ leukocytes counts, High and dominant presence of splenic IAb+CD19+CD80+ antigen-presenting cells counts and capacity of spleen cell to produce high levels of IL-6, TNF-?, IFN-? and lower levels of IL-10 early after tumor cells implantation; rapid T-cell polarization to secret high quantities of Th1 type cytokine IFN-? and low quantities of Th2 type cytokine IL-10; rapid generation and greater numbers of CD4+ and CD8+ activated T cells expressing CD45RB or CD44 markers; and also CD4+ and CD8+ CD44high or CD44highCD62Llow effector T cells. Herein, IL-2 induced splenic LAK cells from 5-LO KO mice, compared with splenic LAK cells from WT mice, were more efficient at killing B16-F0 melanoma cells. The increased B16-F0 melanoma cells killing activity were also found by treatment of splenic LAK cells from WT mice with a 5-LO activity inhibitor, MK886. Our findings suggest that 5-LO deficiency altered antigen-presenting cells profile, IFN-? and IL-10 production during skin cancer disease favoring the generation of protective immune responses and also provide evidence that 5-LO-derived LTs negatively affect the host survival during experimental B16-F0 melanoma.
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Sánchez-Guajardo, Vanesa María. "Kinetics and competitive capacities of Th1 vs. Th2 CD4+ T cells : the role of Stat6 and Stat4 in CD4+ T cell homeostasis." Paris 6, 2005. http://www.theses.fr/2005PA066547.

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Phillips, Aled Myrddin. "The expression of Th1, Th2 and Treg associated transcription factors in bronchoalveolar cells from patients with sarcoidosis." Thesis, University of Cambridge, 2010. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.608614.

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Dodd, Christopher H. "Toll-like receptor stimulation can lead to differential production of IL-23 and IL-12." Thesis, Birmingham, Ala. : University of Alabama at Birmingham, 2008. https://www.mhsl.uab.edu/dt/2009r/dodd.pdf.

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Coquerelle, Caroline. "Contrôle des réponses immunitaires de type Th1 par les lymphocytes T régulateurs naturels et induits." Doctoral thesis, Universite Libre de Bruxelles, 2008. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/210397.

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Depuis leur découverte en 1973 par Steinman et Cohn, le rôle des cellules dendritiques dans l’initiation des réponses immunitaires a largement été documenté. En effet, les cellules dendritiques constituent les cellules présentatrices d’antigènes professionnelles capables de détecter des molécules microbiennes et inflammatoires afin d’activer le système immunitaire. Outre leur implication dans l’induction des réponses immunes, de plus en plus d’études suggèrent que les cellules dendritiques interviennent dans le contrôle des réponses immunitaires via la sécrétion de cytokines anti-inflammatoires et/ou l’activation ou l’induction de lymphocytes T régulateurs. Ceux-ci incluent les cellules T régulatrices issues naturellement du thymus et les cellules T régulatrices induites en périphérie. <p><p>Des résultats obtenus au sein de notre laboratoire ont mis en évidence l’importance des cellules T régulatrices dans le contrôle des réponses de type Th1 induites à l’aide de cellules dendritiques matures chargées avec des antigènes étrangers. Nous avons, dès lors, étudié le rôle du récepteur CTLA-4 exprimé constitutivement à la surface des cellules T régulatrices dans le contrôle des réponses immunitaires induites à l’aide de cellules dendritiques matures et dans un modèle d’inflammation intestinale. L’injection d’anticorps anti-CTLA-4 induit in vitro et in vivo une inhibition de la production d’IFNγ et protège les souris de la colite pro-Th1 induite par l’instillation de TNBS. Cette protection corrèle étroitement avec l’induction de lymphocytes T régulateurs exprimant fortement la molécule ICOS et sécrétant de l’interleukine 10. De plus, nos résultats suggèrent que l’interleukine 10 et l’indoléamine 2, 3 dioxygénase seraient impliquées dans la fonction régulatrice des lymphocytes T ICOShigh. <p><p>Nous avons également analysé les mécanismes impliqués dans le contrôle des réponses de type Th1 par les lymphocytes T régulateurs naturels. Nos résultats suggèrent une régulation différente des réponses Th1 en présence et en absence de cette population régulatrice. En effet, les réponses Th1 sont dépendantes de l’interleukine 12 en présence de lymphocytes T régulateurs naturels, alors qu’en leur absence, la molécule CD70 est requise. <p><p>En conclusion, nos résultats suggèrent que les lymphocytes T régulateurs naturels et induits contrôlent les réponses immunes de type Th1. Au cours de ce travail, nous avons mis en évidence des stratégies distinctes par lesquelles ces deux populations régulatrices contrôlent la réponse immune. Ces résultats complètent la compréhension des mécanismes de régulation du système immunitaire et ouvrent de nouvelles perspectives d’approche immunothérapeutique.<p><br>Doctorat en Sciences<br>info:eu-repo/semantics/nonPublished
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Ramos, Orivaldo Pereira [UNESP]. "Influência das células dendríticas das placas de peyer na modulação das repostas Th1/Th2 em camundongos infectados com Yersinia pseudotuberculosis." Universidade Estadual Paulista (UNESP), 2009. http://hdl.handle.net/11449/103336.

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Made available in DSpace on 2014-06-11T19:32:41Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-01-20Bitstream added on 2014-06-13T21:04:28Z : No. of bitstreams: 1 ramos_op_dr_arafcf.pdf: 948525 bytes, checksum: 0581866624e7c3f57ffffca838856184 (MD5)<br>Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)<br>Yersinia pseudotuberculosis e Y. enterocolitica são patógenos que causam desordens gastrintestinais. Estudos utilizando infecção in vitro demonstraram que Y. enterocolitica pode ter como alvo as células dendríticas (DCs), afetando várias de suas funções, incluindo sua maturação e produção de citocinas, e, conseqüentemente, contribuindo para a diminuição da ativação de células T CD4+. O objetivo deste estudo foi investigar o papel das células dendríticas das placas de Peyer (PP) na determinação do padrão de resposta imune, Th1 e Th2, durante a infecção por via intragástrica de camundongos suscetíveis (BALB/c) e resistentes (C57BL/6) com a amostra virulenta de Y. pseudotuberculosis (YpIII pIB1 – Yp+) ou seu par isogênico, curado do plasmídeo de virulência (YpIII – Yp-). As DCs das PP foram obtidas no 1°, 3° e 5° dia pós-infecção, quantificadas e analisadas quanto às suas subpopulações, expressões de moléculas de superfície e capacidade imunoestimulatória por citometria de fluxo, e quanto à secreção de citocinas (IL-4, IL-10, IL-12 e TNF-α) por ELISA. Os linfócitos das PP também foram obtidos no mesmo período e tiveram suas sub-populações e o padrão de citocinas intracelulares Th1/Th2 (IL-2, IL-4, IL-10 e IFN-γ) analisado por citometria de fluxo. A infecção por Yp+ reduziu o número de DCs no 1° dia pós-infecção e aumentou, no período inicial, a expressão de B7.1 e B7.2 nos camundongos BALB/c. Nos camundongos C57BL/6 reduziu o número de DCs durante todo o período analisado, aumentou a expressão de B7.1 e B7.2 no período inicial e a expressão de ICAM-1. A infecção por ambas as amostras provocou redução da sub-população CD8α+ e da expressão de MHC II nas duas linhagens de animais, aumentou a sub-população CD11b+ nos animais suscetíveis e diminuiu nos animais resistentes. Os animais estudados não apresentaram...<br>Yersinia pseudotuberculosis and Y. enterocolitica are pathogens that cause gastrointestinal disorders. Studies using in vitro infection demonstrated that Y. enterocolitica can have as a target dendritic cells (DCs), affecting several of its functions, including their maturation and production of cytokines, and, consequently, contributing to the diminished activation of the T CD4+ cells. The aim of this study was to investigate the role of dendritic cell from Peyer’s patches (PP) in determining of immune response pattern, Th1 and Th2, during infection by the intragastric route in susceptible (BALB/c) and resistant (C57BL/6) mice with a virulent sample of Yersinia pseudotuberculosis (YpIII pIB1 – Yp+) or its isogenic pair, cured of the virulence plasmid (YpIII – Yp-). The PP DCs were obtained on the 1st, 3rd and 5th days postinfection, quantified and analyzed as far as their subpopulations, expressions of surface molecules and immunostimulatory capacity by flow cytometry, and the cytokines secretion (IL-4, IL-10, IL-12 and TNF-α) by ELISA. The PP lymphocytes were also obtained in the same period, and had their subpopulations and the pattern of intracellular Th1/Th2 cytokines (IL-2, IL-4, IL-10 and IFN-γ) analysed by flow cytometry. The infection by Yp+ reduced the number of DCs on the 1st day post-infection and increased, in the initial period, the expression of B7.1 and B7.2 in BALB/c. In C57BL/6 mice reduced the number of DCs throughout the study period, increased the expression of B7.1 and B7.2 in the initial period and the expression of ICAM-1. The infection by both samples reduced CD8α+ subpopulation and expression of MHC II in both animals, increased CD11b+ sub-population in susceptible animals and reduced the same sub-population in resistant animals. The studied animals did not present important differences as far as secretion of cytokines by the DCs of PP and both... (Complete abstract click electronic access below)
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Mardahl, Maibritt [Verfasser]. "Molecular regulation of P-selectin ligand in TH1 and TH2 cells in vitro, crucial for the homing of CD4+ T cells into inflamed tissue / Maibritt Mardahl." Berlin : Freie Universität Berlin, 2016. http://d-nb.info/1117028429/34.

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Lucas, Casaca Vera Isabel. "Role of Th1 and Th2 cell-specific polymorphisms and of Regulatory T cells modulated by farm exposure for the determination of childhood allergic diseases." Diss., Ludwig-Maximilians-Universität München, 2014. http://nbn-resolving.de/urn:nbn:de:bvb:19-172198.

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Summary: Allergic diseases have exponentially increased during the last decades. The complexity of its aetiology is due to multifaceted interactions between genetic and environmental factors on the development of the immune system. While advances of technology have identified allergy susceptibility genes, functional assays are needed to better understand the underlying mechanisms. Epidemiological studies have consistently shown that rural/farm environments are protective for the development of allergic diseases, including asthma and atopic sensitization. Importantly, prenatal and early life exposures have been shown to confer the strongest protection effects. The mechanisms of how farming modulates the immune system are still not disentangled in detail but include regulation of innate receptors and Regulatory T cells. In the herewith presented thesis, the following main findings were achieved in the context of genetic and immunological influences on development of allergic disease in two different birth cohort studies: First, 200 neonates were assessed for genetic influence of polymorphisms on neonatal immune responses and development of allergic diseases in childhood. The present study suggested a role for polymorphisms in the Th2-pathway, particularly for STAT6 rs324011, on immune regulation at an early stage of immune maturation, namely significantly lower Treg-associated gene expression and Th1-polarization. Polymorphisms in the Th1-pathway, namely the transcription factors TBX21 and HLX1, were shown to be relevant in shaping early immune responses and mainly Th2 cytokines at birth. Th1 and Th2 genotype-related immune responses at birth were partially associated with development of allergic diseases and/or protection during early life. These children are currently followed until the age of 6 years to further investigate allergic and respiratory disease during age-related immune maturation. Secondly, almost 150 children were investigated at the age of 6 years to assess the role of regulatory T cells in relation to farm exposures and clinical outcomes of allergic diseases. Our data indicated an inverse association of farm exposures and the prevalence of asthma during childhood. Children exposed to hay, stable and farm milk had a lower prevalence of asthma. Regarding underlying immune mechanisms, we have detected that children with contact to hay have increased levels of Treg cells and that farm milk intake earlier during childhood can still be partially reflected on Treg cells levels at age 6 years. Assessing Treg functional mechanisms, changes in cytokine secretion were observed depending on the farming and asthmatic status of the children, however confirmation in a larger number of children is required In summary the present work indicated that Th1 and Th2 polymorphisms were associated with modulated immune responses already at birth and influenced allergic disease development during the first three years of life. Furthermore, farm exposures were associated with a lower prevalence of asthma and associated with modulation of regulatory T cell frequency in German children at age 6 years.
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32

Abdulaal, Wesam. "The role of Interleukin-1 signaling in the immune defense and in the development of the T helper cell lineage." Thesis, University of Manchester, 2015. https://www.research.manchester.ac.uk/portal/en/theses/the-role-of-interleukin-1-signaling-in-the-immune-defense-and-in-the-development-of-the-t-helper-cell-lineage(1432f7f4-7c04-4bc5-9fda-4441b5c14e66).html.

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IL-1 is a pro-inflammatory cytokine which play an important role in the activation and regulation of host defence and immune responses to inflammation or injury. IL-1 is able to bind and activate IL1-RI and IL1-RII, which are found on many cells types. The role of the IL-1 signalling in the deployment of Th cell subsets, especially Th17 cells is well known. However, the specific cells which are responsible for the expression of IL-1 signalling in the immune defense and in the development of the Th cell lineage in response to infection, is still largely unclear. Therefore in this thesis, IL1-RI conditional knockout mice specifically in hematopoietic cells (IL1-RI vaviCre+) were generated. Using IL1-RI vaviCre+ mice in comparison with IL1-RI global knockout mice (IL1-RI-/-) would determine whether the expression IL-1 signalling from hematopoietic cells is responsible for the immune defense and in the development of the Th1, Th2 and Th17 cells against gastrointestinal helminth Trichuris muris (T.muris) infections. The generation of IL1-RI vaviCre+ mice have been investigated at the genomic and proteomic level in order to confirm that the Il1-rI gene is inactivated in hematopoietic cells. The characterisation of IL1-RI vaviCre + mice at the genomic level confirmed that the Il1-rI gene was obliterated successfully. At protein level the characterisation of IL1- RI vaviCre + mice confirmed that IL1-RI was dysfunctional in hematopoietic cells. Additionally, the development of the immune cells was investigated in IL1-RI vaviCre + and IL1-RI-/- mice. Our findings demonstrated that the lymphocyte development was not affected by the deletion of the IL1- RI gene. This data indicated that IL1- RI vaviCre + and IL1-RI-/- mice are vital in vivo models. In high dose infection, both IL1-RI vaviCre + and IL1-RI -/- mice were able to clear the infections due to their ability to generate a Th2 response. Both IL1-RI vaviCre + and IL1-RI -/- mice infected with low dose of T.muris were susceptible to infections and showed high levels of Th1 cytokines. Thus, we hypothesised that IL1-RI signalling in hematopoietic cells was not required for worm expulsion and the generation of Th2 and Th1 response. Interestingly, low dose T.muris infection showed a clear reduction in the Th17 cytokines IL22 and IL17 in both IL1-RI vaviCre + and IL1-RI -/- mice, suggesting that IL-1 signalling expressed from hematopoietic cells is responsible for the development of Th17 cells and secretion of IL17 and IL22. IL1- RI vaviCre + and IL1-RI -/- mice infected with low dose of T.muris also showed an increase in inflammation in the colon and decreased of goblet cell hyperplasia. It is well known that IL22 plays an important role in preventing tissue damage and repair. Thus, in this study IL22 global knockout mice (IL22 -/-) were used to determine if the change in crypt lengths and goblet cell hyperplasia in IL1-RI vaviCre + and IL1-RI -/- was due to an absence of IL22. Our finding showed that IL22 -/- mice infected with low dose of T.muris had increased crypt length and a reduction in goblet cells. The similar phenotype in crypt length and goblet cell hyperplasia between IL22 -/-, IL1-RI vaviCre + and IL1-RI -/- mice suggested that a lack of IL22 in IL1-RI vaviCre + and IL1-RI -/- mice is responsible for the change in mice phenotype. It also provides more evidence for the role of IL-1 signaling in hematopoietic cells in the generation of Th17 cells and in the production of its cytokine IL22.IL1-RII is an inhibitor of IL1-RI, thus, in this study IL1-RII global knockout mice (IL1-RII -/-) mice was used in comparison with IL1-RI -/- mice to verify the role of IL-1 signaling in the development of Th17 cells. Our finding showed an overexpression of IL17 and IL22 in IL1-RII -/- compared with IL1-RI -/- mice and a higher level of IL17 in IL1-RII -/- mice compared with IL1-RII flox/flox mice. This data confirmed that IL-1 signaling is important for the development of Th17 cells and the production of its cytokine IL17 and IL22.
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33

Pressley, Jennifer Sparkman. "Immune Cell Subsets Direct or Antagonize Tumor Immunity: Promotion of TH1 Responses in Tumor Vaccination." Thesis, Virginia Tech, 2005. http://hdl.handle.net/10919/33509.

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Tumors evade immune system tumor-controlling functions. T cells critical to antitumor immunity are tolerogenic in tumor-burdened animals, and fail to lyse neoplastic cells. Our goal was to investigate the kinetics of immune dysfunction related to tumor-burdened host (TBH) memory T cell responses (or the lack thereof). We demonstrate tumor growth impairs T cell activation by modulating CD4+ T cell infiltration and systemic CD44 and CD62L activation marker expression, and by downregulating TBH TH1 cytokine production by splenic CD4+ T cells. Since chemotherapeutic treatments have potent cytostatic effects, we posited they enhance T cell dysfunctionality; which leads to limited therapeutic efficacy. Paclitaxel is a potent chemotherapeutic agent currently being administered in Stage III clinical trials; however, it reduces T cell proliferative capacity and interferon-γ (IFN-γ) production. In contrast, our data suggest that administration of low dose paclitaxel prolongs adaptive immunity in a limited capacity. We show paclitaxel enhances CD4highCD62Llow cell populations that drive TH1 cytokine production and prolongs the production of interleukin-2 (IL-2) in TBHs. We hypothesize that the initiation and maintenance of activated TH1 cell populations in patients during therapy serves as a reliable prognostic indicator of a favorable therapeutic response. Paclitaxel's limited therapeutic effects are due, in part, to its suppression of T cell activities; but the administration of low dose chemotherapy in combination with immunotherapeutic agents temporally takes advantage of paclitaxel's immunostimulatory capabilities. Our work will enhance current understanding of immune dysregulation during cancer development, and promote advances in the monitoring and development of combinatorial cancer treatments.<br>Master of Science
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Schenk, Michael Peter. "Platelets promote immunopathology in Plasmodium berghei infection by inhibiting the development of Interleukin-10 expressing Th1 cells." Thesis, University of Reading, 2013. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.590145.

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Currently there are 3.3 billion people world -wide at risk of contracting malaria with the species Plasmodium falciparum being responsible for around 1 million deaths annually. P. Falciparum causes a symptom known as cerebral malaria (CM) which, if not treated quickly results in an unrousable coma which can lead to death with in 24-72 hours. With the use of mouse malaria models, the causes of CM are becoming clearer and currently it is understood to be caused by the sequestration of parasitized red blood cells, leukocytes and plate lets with in the microvasculature within the cerebral cortex. This sequestration is linked to inflammation with IFNy and TNFa being key initiators in promoting CM pathology. Although platelets sequester with in the cerebral cortex and malaria is usually accompanied by thrombocytopenia; however, a link between platelets and pathology has never been fully established. The data in this study demonstrates that an increase in parasite biomass is thrombocytopenia and that both parasitaemia and thrombocytopenia are linked to pathology in malaria. The data in this report also shows that mice are rescued from associated malaria pathology when platelets are depleted or inhibited. Analysing splenic leukocyte populations, our data demonstrated that the source of the increase in plasma concentrations of IL-IO and IFNy in P. berghei-infected platelet-depleted mice as shown by Van der Heyde et al. is possibly down to the increase in activated IFNy-expressing Th1 cells. Platelet depletion or platelet antagonist treatment in P. berghei infected also results in an increased population of IL-lO-producing Th2 and self-limiting IL-10-producing Thl cells that have been shown to be crucial in preventing immunopathology. This increase in the expansion of Thl and Th2 populations in response to P. berghei infection is not mediated by the antigen presenting cell populations, as they population and their maturity appears to be un-affected by either platelet depletion or platelet inhibition.
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Malbec, Agathe. "Contrôle épigénétique de la biologie des lymphocytes T CD4." Thesis, Toulouse 3, 2018. http://www.theses.fr/2018TOU30305/document.

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Les lymphocytes T CD4 naïfs sont des cellules plastiques, capables de moduler finement leur programmation selon les signaux environnementaux qu'ils intègrent. Ils adaptent ainsi leur phénotype et leur fonction au type de danger Lors d'une infection par un agent pathogène intracellulaire par exemple, ils acquièrent un phénotype Th1 sous l'influence de médiateurs solubles tels que l'IL-12 et l' IFN-γ. Ces signaux mobilisent un set restreint de facteurs de transcription, coordonné par Tbet, qui programment la cellule afin qu'elle induise l'élimination du danger par des mécanismes impliquant une production massive d'IFN-γ. En réponse à des allergènes ou à des parasites extracellulaires, les lymphocytes T peuvent aussi acquérir un phénotype Th2, caractérisé par l'expression du facteur de transcription Gata-3 et par la production d'IL-4, d'IL-5 et d'IL-13. Afin de garantir la stabilité des lignages, ces processus de différenciation peuvent s'accompagner d'une perte de potentialité. Contrairement aux cellules T naïves, les cellules Th1 sont par exemple incapables d'allumer le programme d'expression génique Th2 en présence d'IL-4, et les lymphocytes Th2 verrouillent le programme Th1. Si nous savons aujourd'hui que l'acquisition des fonctions effectrices, comme l'équilibre entre détermination cellulaire et plasticité, sont régulés par des mécanismes épigénétiques, la plupart des acteurs moléculaires qui contrôlent la programmation des lymphocytes T au niveau de la chromatine reste encore à identifier. Durant ma thèse, j'ai étudié le rôle de la lysine méthyltransférase SETDB1, qui catalyse la di- ou tri-méthylation de la lysine 9 de l'histone 3 (H3K9me3), dans la différenciation des lymphocytes T CD4. Il avait déjà été proposé qu'H3K9me3 ait un impact sur la programmation de ces cellules en réponse aux signaux de l'environnement, mais personne n'avait encore étudié le rôle de SETDB1 dans ces processus lorsque j'ai commencé ma thèse. A l'aide d'une lignée murine déficiente pour SETDB1 spécifiquement dans les lymphocytes T, nous avons montré in vitro et in vivo que la balance Th1/Th2 est fortement augmentée en l'absence de l'enzyme, et que cette dérégulation résulte d'une perte de répression du réseau génique Th1. [...]<br>Upon activation, naïve CD4 T cells differentiate into distinct helper or regulatory T cell subsets depending on environmental signals received. This process relies on complex and lineage-specific gene expression programs whose dynamics and stability are regulated at the level of the chromatin. The epigenetic pathways involved, however, remain largely unknown. Here, we report that the histone methyltransferase SETDB1 critically controls the Th1 gene expression program. SETDB1-deficient naïve CD4 T cells show exacerbated Th1 priming, and when exposed to a Th1-instructive signal, SETDB1-deficient Th2 cells cross lineage boundaries and transdifferentiate into Th1 cells. Surprisingly, SETDB1 does not appear to control Th1 gene promoter activity. Instead, it deposits the repressive H3K9me3 mark at a restricted and cell-type specific set of endogenous retroviruses (ERVs) strongly associated with genes involved in immune processes. Refined bioinformatic analyses indicated that these retrotransposons either flank and repress Th1 gene cis-regulatory elements or behave themselves as Th1 gene enhancers. In conclusion, H3K9me3 deposition by SETDB1 ensures T cell lineage integrity by repressing a repertoire of ERVs that have been exapted into cis-regulatory modules to shape and control the Th1 gene network
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Ellison, Cynthia A. "The role of NK1.1§+ cells and TH1 cytokines in the pathogenesis of acute murine graft-versus-host disease (GVHD)." Thesis, National Library of Canada = Bibliothèque nationale du Canada, 1998. http://www.collectionscanada.ca/obj/s4/f2/dsk2/tape17/PQDD_0023/NQ32880.pdf.

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37

Tupin, Emmanuel. "Immunomodulation of atherosclerosis : impact of Th balance and CD1d-restricted NKT cells." Stockholm, 2004. http://diss.kib.ki.se/2004/91-7140-128-8/.

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38

Klein, Sebastian [Verfasser]. "Modulation of the TH1/TH2 differentiation by B cells, C5aR1 and CD154 in antigen dose dependent mouse models / Sebastian Klein." Lübeck : Zentrale Hochschulbibliothek Lübeck, 2018. http://d-nb.info/1153039354/34.

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39

Lu, Tangying (Lily). "Cannabinoids suppress dendritic cell-induced T helper cell polarization." [Tampa, Fla] : University of South Florida, 2006. http://purl.fcla.edu/usf/dc/et/SFE0001790.

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40

Medina, Tiago da Silva. "Participação do eixo Th17/IL-27 no controle da infecção experimental com Trypanosoma cruzi." Universidade de São Paulo, 2014. http://www.teses.usp.br/teses/disponiveis/17/17147/tde-02052014-160055/.

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Produzida por macrófagos e células dendríticas, a IL-27 é uma citocina heterodimérica capaz de induzir células Tr1 produtoras de IL-10 e consequentemente regular linfócitos Th1, Th2 e Th17, dependendo da doença envolvida. Partindo-se do pressuposto de que a infecção causada por Trypanosoma cruzi normalmente induz miocardite refletida pela migração intensa de linfócitos Th1 para o tecido cardíaco, nós analisamos o papel regulador da IL-27 nesta condição inflamatória. Nós inicialmente verificamos que a IL-27 foi prontamente induzida in vitro em células infectadas com T. cruzi. Para gerar miocardite intensa coordenada por linfócitos Th1, nós polarizamos linfócitos T naïves para o padrão Th1 na ausência de moléculas relacionadas ao perfil Th17 (camundongos IL-17R-/-, IL-23-/- e IL-6-/-). Como esperado, a inflamação cardíaca intensa e o dano tecidual foram observados na ausência das moléculas do padrão Th17, o que contribuiu para a morte prematura dos animais IL-17R-/-, IL-23-/- e IL-6-/-, precisa e notoriamente pela indução da migração excessiva de linfócitos Th1 para o tecido cardíaco via CXCL-9 e CXCL-10. Para explorar os mecanismos pelos quais a IL-27 controla a miocardite induzida pelo T. cruzi, nós encontramos um recrutamento substancial de macrófagos produtores de IL-27 para o tecido cardíaco, o qual foi mediado pelas quimiocinas CCL3 e CCL4 na ausência de moléculas do padrão Th17. Para determinar quais os receptores necessários para a produção de IL-27, nós observamos que macrófagos derivados da medula óssea de camundongos deficientes de TLR4-/-, TLR9-/- e NLRP3-/- aboliram completamente a produção desta citocina após a infecção in vitro com T. cruzi, enquanto o receptor TLR2 foi dispensável. Nós também verificamos que macrófagos produtores de IL-27 suprimiram linfócitos Th1 através da indução de células Tr1 produtoras de IL-10 após a infecção com T. cruzi. Em seguida, nós avaliamos se a IL-27 foi correlacionada com a proteção cardíaca durante a doença de Chagas. Nós observamos níveis séricos elevados de IL-27 tanto em pacientes com a forma clínica indeterminada ou cardíaca leve, enquanto pacientes com cardiomiopatia moderada ou grave produziram níveis reduzidos de IL-27. Neste estudo, nós descrevemos um novo mecanismo regulador desempenhado por macrófagos produtores de IL-27 no controle da miocardite induzida por T. cruzi. Macrófagos produtores de IL-27 podem suprimir processos inflamatórios desencadeados por linfócitos Th1, os principais vilões na doença de Chagas.<br>IL-27 is a heterodimeric cytokine produced by macrophages and dendritic cells known to induce IL-10-producing Tr1 cells and to regulate Th1, Th2, and Th17 lymphocytes, depending on the underlying disease. Because the infection caused by Trypanosoma cruzi normally induces myocarditis mirrored by an outstanding migration of Th1 cells to the heart tissue, we analyzed the regulatory role of IL-27 in this inflammatory condition. We firstly verified that IL-27 was promptly induced by in vitro T. cruzi-infected spleen cells. To generate a robust myocarditis coordinated by Th1 lymphocytes, we polarized lymphocytes to a Th1 pattern by infecting mice in the absence of Th17-related molecules (IL-17R-/-, IL-23-/-, and IL-6-/- mice). As expected, an impressive cardiac inflammation and damage was observed in the absence of Th17-related molecules, leading IL-17R-/-, IL-23-/-, and IL-6-/- mice to the premature death, precisely and notably by inducing an exuberant Th1 migration to the heart tissue via CXCL9 and CXCL10 chemokines. To explore the mechanisms by which IL-27 controls T. cruzi-induced myocarditis, we found a striking recruitment of IL-27-producing macrophages to the heart tissue mediated by increased levels of CCL3 and CCL4 chemokines in the absence of Th17-associated molecules. To gain further insights into the receptors required to IL-27 production, we observed that bone marrow-derived macrophages from TLR4-/-, TLR9-/-, and NLRP3-/- mice completely abolished IL-27 production after in vitro T. cruzi infection, while TLR2 was dispensable. We also verified that IL-27-producing macrophages supressed Th1 lymphocytes by inducing IL-10-producing Tr1 cells after T. cruzi infection. We next assessed whether IL-27 was correlated to cardiac protection during Chagas Disease. We observed augmented serum levels of IL-27 in either patients with indeterminate (asymptomatic) form or mild cardiac form, whereas patients with moderate or severe cardiomyopathy were poor producers of IL-27. Here, we described a novel regulatory mechanism developed by IL-27-producing macrophages in the control of T. cruzi-induced myocarditis. IL-27-producing macrophages can suppress inflammatory processes caused by Th1 lymphocytes, the bona fide culprits of Chagas Disease.
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41

Ramos, Orivaldo Pereira. "Influência das células dendríticas das placas de peyer na modulação das repostas Th1/Th2 em camundongos infectados com Yersinia pseudotuberculosis /." Araraquara : [s.n.], 2009. http://hdl.handle.net/11449/103336.

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Orientador: Beatriz Maria Machado de Medeiros<br>Banca: Beatriz Maria Machado de Medeiros<br>Banca: Maria Terezinha Serrão Peraçoli<br>Banca: Iracilda Zeppone Carlos<br>Banca: Cleni Mara Marzocchi Machado<br>Banca: Fernanda de Freitas Anibal<br>Resumo: Yersinia pseudotuberculosis e Y. enterocolitica são patógenos que causam desordens gastrintestinais. Estudos utilizando infecção in vitro demonstraram que Y. enterocolitica pode ter como alvo as células dendríticas (DCs), afetando várias de suas funções, incluindo sua maturação e produção de citocinas, e, conseqüentemente, contribuindo para a diminuição da ativação de células T CD4+. O objetivo deste estudo foi investigar o papel das células dendríticas das placas de Peyer (PP) na determinação do padrão de resposta imune, Th1 e Th2, durante a infecção por via intragástrica de camundongos suscetíveis (BALB/c) e resistentes (C57BL/6) com a amostra virulenta de Y. pseudotuberculosis (YpIII pIB1 - Yp+) ou seu par isogênico, curado do plasmídeo de virulência (YpIII - Yp-). As DCs das PP foram obtidas no 1°, 3° e 5° dia pós-infecção, quantificadas e analisadas quanto às suas subpopulações, expressões de moléculas de superfície e capacidade imunoestimulatória por citometria de fluxo, e quanto à secreção de citocinas (IL-4, IL-10, IL-12 e TNF-α) por ELISA. Os linfócitos das PP também foram obtidos no mesmo período e tiveram suas sub-populações e o padrão de citocinas intracelulares Th1/Th2 (IL-2, IL-4, IL-10 e IFN-γ) analisado por citometria de fluxo. A infecção por Yp+ reduziu o número de DCs no 1° dia pós-infecção e aumentou, no período inicial, a expressão de B7.1 e B7.2 nos camundongos BALB/c. Nos camundongos C57BL/6 reduziu o número de DCs durante todo o período analisado, aumentou a expressão de B7.1 e B7.2 no período inicial e a expressão de ICAM-1. A infecção por ambas as amostras provocou redução da sub-população CD8α+ e da expressão de MHC II nas duas linhagens de animais, aumentou a sub-população CD11b+ nos animais suscetíveis e diminuiu nos animais resistentes. Os animais estudados não apresentaram... (Resumo completo, clicar acesso eletrônico abaixo)<br>Abstract: Yersinia pseudotuberculosis and Y. enterocolitica are pathogens that cause gastrointestinal disorders. Studies using in vitro infection demonstrated that Y. enterocolitica can have as a target dendritic cells (DCs), affecting several of its functions, including their maturation and production of cytokines, and, consequently, contributing to the diminished activation of the T CD4+ cells. The aim of this study was to investigate the role of dendritic cell from Peyer's patches (PP) in determining of immune response pattern, Th1 and Th2, during infection by the intragastric route in susceptible (BALB/c) and resistant (C57BL/6) mice with a virulent sample of Yersinia pseudotuberculosis (YpIII pIB1 - Yp+) or its isogenic pair, cured of the virulence plasmid (YpIII - Yp-). The PP DCs were obtained on the 1st, 3rd and 5th days postinfection, quantified and analyzed as far as their subpopulations, expressions of surface molecules and immunostimulatory capacity by flow cytometry, and the cytokines secretion (IL-4, IL-10, IL-12 and TNF-α) by ELISA. The PP lymphocytes were also obtained in the same period, and had their subpopulations and the pattern of intracellular Th1/Th2 cytokines (IL-2, IL-4, IL-10 and IFN-γ) analysed by flow cytometry. The infection by Yp+ reduced the number of DCs on the 1st day post-infection and increased, in the initial period, the expression of B7.1 and B7.2 in BALB/c. In C57BL/6 mice reduced the number of DCs throughout the study period, increased the expression of B7.1 and B7.2 in the initial period and the expression of ICAM-1. The infection by both samples reduced CD8α+ subpopulation and expression of MHC II in both animals, increased CD11b+ sub-population in susceptible animals and reduced the same sub-population in resistant animals. The studied animals did not present important differences as far as secretion of cytokines by the DCs of PP and both... (Complete abstract click electronic access below)<br>Doutor
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42

Hull, Dobrina Nikolaeva. "The dynamics of Th17 and Th1 cells during anti-TNF therapy in patients with inflammatory arthritis and relationship with treatment response." Thesis, Imperial College London, 2013. http://hdl.handle.net/10044/1/29116.

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Anti-TNF agents have revolutionised the treatment of rheumatoid arthritis (RA), ankylosing spondylitis (AS) and psoriatic arthritis (PsA), however a significant proportion of patients respond inadequately. Studies in murine and human arthritis have paradoxically shown that anti-TNF treatment can increase circulating Th17 and Th1 cells but the relationship of these changes to treatment response remains unclear. The aim of the work in this thesis was to conduct a prospective, longitudinal investigation of patients with inflammatory arthritis during anti-TNF treatment and using clinical, ultrasound and immunological assessments to gain an understanding of the immune correlates of treatment response. Patients with RA (n=25), AS (n=15) and PsA (n=8) were recruited and followed over the first 12 weeks of treatment. Improvement in validated disease activity scores defined treatment responders and non-responders. Power Doppler ultrasound (PDUS) provided a quantitative assessment of changes in synovial thickening and vascularity during treatment, with synovial vascularity showing faster and greater reduction with treatment than synovial thickening. PBMCs testing using IL17 and IFNy ELISpot assays and flow cytometry consistently showed increased frequencies of circulating Th1 and Th17 cells in all three disease groups during anti-TNF therapy. Multiplex cytokine testing demonstrated a decrease in serum levels of proinflammatory cytokines and chemokines. Analyses of relationships between clinical, ultrasonographic and T-cell immunological changes revealed significant negative correlations between the increased frequency of Th1 and Th17 cells and reduction in synovial thickening and vascularity from baseline to 12 weeks on treatment in the RA group. Higher numbers of circulating Th17 cells at baseline in the RA group were associated with poorer anti-TNFa treatment response as defined by DAS28 score and ultrasonographic measures. This is the first study to link changes in T-cell immunopathology evaluated by cellular assays with morphological changes in arthritis assessed by PDUS during anti-TNFa treatment.
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43

Radbruch, Andreas [Gutachter], Chiara [Gutachter] Romagnani, and Hans-Dieter [Gutachter] Volk. "Role of Twist1 in metabolism of repeatedly stimulated Th1 cells / Gutachter: Andreas Radbruch, Chiara Romagnani, Hans-Dieter Volk." Berlin : Humboldt-Universität zu Berlin, 2019. http://d-nb.info/119934043X/34.

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44

SARGENTINI, VALERIA. "Activated T lymphocytes instruct monocytes to differentiate into inflammatory dendritic cells in a feedback control of human Th1/Th2 responses." Doctoral thesis, Università degli Studi di Roma "Tor Vergata", 2009. http://hdl.handle.net/2108/988.

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Le cellule dendritiche (DCs) rappresentano una popolazione di cellule eterogenea con diversa origine, fenotipo e funzione che svolge un ruolo chiave nell' induzione, coordinazione e mantenimento delle risposte immunitarie adattative. La maggior parte delle conoscenze riguardanti le DCs sono state acquisite grazie ad esperimenti eseguiti con DCs fatte differenziare in vitro da monociti trattati con diverse combinazioni di citochine; in particolare è ormai noto che i monociti umani differenziano a DCs se coltivati con il fattore di stimolazione di colonie granulocita rie/macrofagiche(GM-CSF) e interleuchina (IL)-4. Tuttavia, la possibilità che i monociti rappresentino i precursori di DCs umane tissutali in condizioni fisiologiche rimane un' ipotesi controversa. Inoltre, non è stato ancora definitivamente stabilito quale sia la popolazione cellulare responsabile della sintesi delle citochine necessarie al differenziamento di monociti in vitro ed in che modo il loro rilascio venga regolato in vivo. In questa tesi viene dimostrato come, in seguito ad attivazione specifica, i linfociti T sono in grado di rilasciare citochine che a loro volta inducono il differenziamento in DCs sia di monociti presentanti l' antigene che di monociti circolanti. In base alla polarizzazione funzionale dei linfociti T attivati, i monociti differenziano in DCs con diverso fenotipo e funzionalità. I monociti esposti alle citochine rilasciate da linfociti T helper (Th) 1 e Th0 differenziano in DCs caratterizzate da una ridotta capacità di captazione e presentazione dell' antigene. Inoltre, queste DCs mostrano una capacità limitata nellâ'indurre una polarizzazione in senso Th1 delle cellule T naive, bensì sono in grado di attivare cellule T naive secernenti IL-10, dimostrando in questo modo un potenziale tollerogenico. Al contrario, DCs derivate da monociti che risentono di citochine rilasciate da linfociti Th2 sono cellule presentanti l' antigene (APC) caratterizzate da una marcata capacità di polarizzazione in senso Th1. Partendo dalla considerazione che i monociti vengono reclutati insieme ai linfociti in siti di infiammazione cronica, i risultati ottenuti in questo lavoro suggeriscono che, in ambienti caratterizzati da un rilascio prevalente di citochine associate a cellule Th1, Th0 o Th2, possono essere generate DCs funzionalmente differenti tra loro. Poiché le capacità dimostrate da queste DCs come cellule presentanti l' antigene hanno conseguenze funzionali opposte, è stato proposto un modello in vitro in grado di riprodurre il contributo delle DCs infiammatorie, derivate da monociti, nella regolazione della risposta immunitaria in atto.<br>Dendritic cells (DCs) are a heterogeneous population of cells with different origin, phenotype and function that share the crucial role of inducing, coordinating and maintaining adaptive immune responses. Most of the knowledge on human DCs relies on experiments performed with DCs differentiated in vitro from monocytes treated with diverse cocktails of recombinant cytokines; in particular it is well established that human monocytes differentiate into DCs when cultured with granulocyte-macrophage colony-stimulating factor and interleukin (IL)-4. However, the possibility that monocytes represent precursors for tissue human DCs under physiological conditions remains controversial. Moreover, it is not completely established which cell population synthesizes the cytokines required for monocyte differentiation in vitro and how their secretion is regulated in vivo. In this thesis is shown that, on specific activation, T lymphocytes are capable of secreting cytokines, which in turn induce the differentiation into DCs of antigen-presenting and bystander monocytes. Depending on the functional polarization of the activated T lymphocytes, monocytes differentiate into DCs with diverse phenotype and functionality. Monocytes exposed to cytokines released by T helper (Th) 1 and Th0 lymphocytes differentiate into DCs with a reduced antigen uptake and antigen presentation capacity. Moreover, these DCs show a limited capacity to induce Th1 polarization of naive T cells but are capable of priming IL-10-secreting T cells, thus displaying tolerogenic potential. Conversely, DCs derived from monocytes sensing cytokines released by Th2 lymphocytes are antigen-presenting-cell (APC) endowed with a marked Th1 polarization capacity. Starting from the point that monocytes are co-recruited with lymphocytes in chronic inflammation sites, the results obtained in this work suggest that functionally different DCs can be generated in environments characterized by the prevalent release of Th1-, Th0-, or Th2-associated cytokines. Because the APC capacities of these DCs showed opposite functional consequences, it has been proposed an in vitro model that can reproduce a contribution in the regulation of the ongoing immune response by monocyte-derived inflammatory DCs.
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45

Holzknecht, Barbara Juliane. "Direkter ex vivo Nachweis Myelin Bacis Protein (MBP)-spezifischer T-Helferzellen bei Multiple Sklerose Patienten." Doctoral thesis, Humboldt-Universität zu Berlin, Medizinische Fakultät - Universitätsklinikum Charité, 2003. http://dx.doi.org/10.18452/14983.

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In der Pathogenese der Multiplen Sklerose (MS) wird autoantigenspezifischen proinflammatorischen T-Helferzellen eine entscheidende Rolle zugeschrieben. Das am meisten untersuchte Autoantigen ist das Myelin Basic Protein (MBP). Bisher waren zum Nachweis autoantigenspezifischer T-Zellen deren Kultur über Tage bis Monate unumgänglich. In dieser Arbeit wurden Methoden zum direkten ex vivo-Nachweis autoreaktiver T-Helferzellen etabliert, die die reaktive Sekretion der proinflammatorischen Zytokine Interferon gamma und Tumor Nekrose Faktor alpha nach sechsstündiger Stimulation nachweisen. Die durchflusszytometrische Analyse antigenreaktiver Zytokinexpression in fixierten Zellen wies eine Sensitivität von 1/10.000 in mononukleären Zellen des peripheren Blutes (PBMC) auf. Es konnten damit bei 34 untersuchten MS-Patienten und 25 gesunden Kontrollpersonen keine MBP-reaktiven T-Helferzellen detektiert werden, während sich die Reaktion auf die beiden Kontrollantigene Tetanus Toxoid und Cytomegalie Virus-Antigen in den beiden Gruppen nicht relevant unterschied. Deshalb wurde in einer anderen Methode reaktiv sezerniertes Zytokin extrazellulär auf lebenden Zellen gebunden und durch einen anschließenden magnetischen Anreicherungsschritt die Sensitivität auf 2/100.000 erhöht. Bei einem von acht MS-Patienten wurde so eine Population MBP-spezifischer Zellen mit einer Ausgangsfrequenz von 2,15/100.000 nachgewiesen. Im Liquor von drei MS-Patienten ließen sich keine MBP-reaktiven proinflammatorischen T-Helferzellen detektieren. Diese Ergebnisse implizieren, dass die Frequenz MBP-spezifischer T-Helferzellen im peripheren Blut und im Liquor der meisten MS-Patienten und Kontrollpersonen geringer ist als die Sensitivität der etablierten Methoden, diese Zellen jedoch bei einigen Patienten in höheren Frequenzen nachgewiesen werden können.<br>Autoantigen-specific proinflammatory T-helper cells are assumed to play an important role in the pathogenesis of Multiple Sclerosis (MS). The most extensively studied autoantigen is Myelin Basic Protein (MBP). To detect autoantigen-specific T-cells, so far these had to be cultured for several days or months. In this work methods for the direct ex vivo detection of autoreactive T-helper cells have been established by detecting the reactive secretion of the proinflammatory cytokines Interferon gamma and Tumor Necrosis Factor alpha after six hour stimulation. The flow cytometric analysis of antigen-reactive cytokine expression in fixed cells showed a sensitivity of 1/10.000 in peripheral blood mononuclear cells (PBMC). With this method there could not be detected any MBP-reactive T-helper cells in 34 MS-patients and 25 healthy controls, whereas the reaction after stimulation with the two control antigens Tetanus Toxoid and Cytomegalovirus antigen did not differ relevantly between the two groups. Therefore in another method the reactively secreted cytokine was bound on the surface of living cells and the sensitivity was then increased to 2/100.000 by following magnetic enrichment. With that, there could be detected a population of MBP-specific cells in one of eight MS-patients with a frequency of 2,15/100.000 in PBMC. There could not be found any MBP-reactive proinflammatory T-helper cells in the cerebrospinal fluid of three MS-patients. Our results suggest that the frequency of MBP-specific T-helper cells in peripheral blood and cerebrospinal fluid is below the employed methods' detection limit in most MS-patients, but seldom these cells can be detected in higher frequencies.
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46

Junior, Samuel de Barros Ferreira. "Modulação da severidade da doença periodontal experimental por células CCR5+." Universidade de São Paulo, 2009. http://www.teses.usp.br/teses/disponiveis/25/25142/tde-02072009-112551/.

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As doenças periodontais (DP) afetam os tecidos de suporte dos dentes e são desencadeadas por micro-organismos gram-negativos anaeróbios presentes no biofilme periodontal. A evolução da doença é influenciada pela resposta inflamatória e imunológica do hospedeiro e envolve a participação de diversos tipos celulares, que atuam no micro ambiente local modulando a resposta do hospedeiro em busca do controle da infecção. Acredita-se que citocinas inflamatórias, quimiocinas e seus receptores estão envolvidos na migração celular para os tecidos periodontais, contudo, pouco se sabe sobre os mecanismos de determinação de resistência ou susceptibilidade às DP; ou no desencadeamento do dano tecidual decorrente da resposta. Neste projeto, avaliou-se o papel das células CCR5+ na DP experimental induzida pela inoculação oral de Aggregatibacter actinomycetemcomitans em camundongos C57BL/6 wild type e camundongos CCR5-knockout. Os resultados mostram que a maioria das células CCR5+ possuem fenótipo compatível com células T do subtipo Th1, devido a co-expressão de CD3 e CXCR3; além de co-expressarem RANKL. Na ausência das células CCR5+, houve uma significativa diminuição da migração de células inflamatórias totais e RANKL+ para os tecidos periodontais, diminuição da reabsorção óssea alveolar, diminuição dos níveis de expressão de citocinas pró-inflamatórias TNF&#945;-, IL-1&#946; e IFN-&#947;, assim como diminuição na expressão de MMP-1, MMP-2 e MMP-13. Sua ausência não interferiu no controle da infecção periodontal apesar da diminuição dos níveis de iNOS. Estes resultados conduzem à conclusão de que a maioria das células CCR5+ são células T do subtipo Th1, que atuam como importantes moduladoras das citocinas TNF&#945;-, IL-1&#946; e IFN-&#947;, das metaloproteinases de matriz MMP-1, MMP-2 e MMP-13, e que também expressam e modulam a expressão de RANKL, tendo participação importante na imunopatogenese da DP experimental, sem interferir no controle da infecção periodontal. Estes fatos tornam as células CCR5+ potenciais alvos para intervenção terapêutica visando ao controle das doenças periodontais.<br>The periodontal diseases (PD) affect the supportive tissues of the teeth and are triggered by periodontopathogens present in the dental biofilm. The clinical outcome is highly influenced by the host inflammatory and immune response with participation of many cellular types, that act in the local microenvironment modulating the host response to control the infection. Inflammatory cytokines, chemokines and its receptors are thought to be involved in the cellular migration to the periodontal tissues, but there is little knowledge about the mechanisms of determination of resistance or susceptibility to the PD and in the triggering of tissue damage by immune response components. This study evaluated the role of CCR5+ cells in the experimental PD induced by oral inoculation of Aggregatibacter actinomycetemcomitans in C57BL/6 wild type mice and CCR5-knockout mice. The phenotypic analysis of inflammatory infiltrate demonstrated that the most of CCR5+ cells coexpress CD3 and CXCR3, suggesting a phenotype compatible with Th1-type cells, and also co-express RANKL. In the absence of CCR5+ cells there was a significant overall reduction of inflammatory cells and RANKL+ cells influx to the periodontal tissues, reduction in the alveolar bone resorption, reduction in the levels of pro-inflammatory cytokines TNF&#945;-, IL-1&#946; and IFN-&#947; expression, as a reduction in the expression of MMP-1, MMP-2 and MMP-13. The absence of CCR5+ cells did not impair the control of periodontal infection, despite the reduction of iNOS levels. In conclusion, these data demonstrate that the most of CCR5+ cells are Th1 cells, which act as important modulators of TNF&#945;-, IL-1&#946; and IFN-&#947;, MMP-1, MMP- 2 and MMP-13 levels, and which also express and modulate the expression of RANKL, playing an important role in the immunopathogenesis of experimental PD, without impairing the control of periodontal infection. These facts point to CCR5+ cells as potentials targets to therapeutic interventions aimed to control periodontal diseases.
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47

Wolf, Susanne. "Neurodegeneration und Neuroprotektion." Doctoral thesis, Humboldt-Universität zu Berlin, Mathematisch-Naturwissenschaftliche Fakultät I, 2001. http://dx.doi.org/10.18452/14688.

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Die Infiltration von T Zellen in das Zentrale Nervensystem (ZNS) ist ein Charakteristikum neuroinflammatorischer Erkrankungen wie der Multiplen Sklerose (MS) und ihrem Tiermodell der experimentellen autoimmunen Enzephalomyelitis (EAE), und führt zur Aktivierung intrinsischer Hirnmakrophagen, den Mikrogliazellen, zu axonaler Schädigung sowie zum Zusammenbruch der Blut-Hirnschranke. Die T Zellen, welche als erste im Gehirn erscheinen, sind vom Subtyp Th1, spezifisch für Bestandteile der Myelinscheide, wie das myelinbasische Protein (MBP), produzieren inflammatorische Zytokine und rekrutieren andere unspezifische T Zellen und Makrophagen. Da sich diese Zellen des Immunsystems gegen körpereigene Bestandteile richten, spricht man von autoreaktiven T Zellen und einer autoimmunen Erkrankung. Im ersten Teil meiner Dissertation habe ich den Einfluss dieser autoreaktiven T Zellen auf den Aktivierungszustand von Mikrogliazellen mit Hilfe muriner Schnittkulturpräparate von Hippocampus und entorhinalem Kortex untersucht, welche den myelinisierten Fasertrakt Tractus perforans mit seinen Ursprungsneuronen und Zielzellen enthielten. Gering aktivierte MBP-spezifische T Zellen induzierten die Expression der Aktivitätsmarker MHC-II und ICAM-1 auf den Mikroglia und die damit verbundene axonale Schädigung (Phagozytose) im gleichen Maße wie hochaktivierte unspezifische T Zellen. Nur Th1 Zellen konnten Mikroglia aktivieren. MBP-spezifische Th2 Zellen hingegen reduzieren die Th1 induzierte Mikrogliaaktivierung (ICAM-1) auf Kontrollniveau. MBP-spezifische Th1 Zellen konnten die Expression von B7 auf Mikrogliazellen modulieren, während die MBP-spezifischen Th2 Zellen diese Eigenschaft nicht besaßen. Durch diese Befunde kann die prominente Rolle von autoreaktiven Th1 Zellen beim Auslösen neuroinflammatorischer Prozesse auf ihre einmalige Fähigkeit, Mikrogliazellen zu aktivieren und deren kostimulatorische Moleküle zu modulieren, zurückgeführt werden. Gleichzeitig bieten die Daten eine mögliche Erklärung für die protektive Rolle von Th2 Zellen bei MS und EAE. Es ist bekannt, dass autoreaktive T Zellen, wie die MBP-spezifischen Th1 Zellen, auch im gesunden Zustand im humanen und murinen T-Zell-Repertoire vorhanden sind. Die physiologische Funktion dieser Zellen ist unklar. Untersuchungen am Nervus opticus sowie im Rückenmark in vivo belegen, dass autoreaktive T Zellen und Makrophagen die Reorganisationsprozesse im ZNS nach traumatischer Schädigung positiv beeinflussen. Diese bei neuroinflammatorischen Erkrankungen so destruktiv wirkenden autoreaktiven T Zellen verhindern nach einem experimentell gesetzten Primärschaden im ZNS das Fortschreiten der Schädigung und es kommt zu einer fast vollständigen Regeneration des Gewebes. Im zweiten Teil meiner Promotionsarbeit habe ich versucht, die Mechanismen, welche hinter dieser Protektion stecken aufzuspüren. Dazu habe ich ebenfalls das in vitro Hirnschnittmodell benutzt. Für diese Fragestellungen wurden Akutschnitte verwendet, die ein Modell für primäre Schädigung im ZNS darstellen. MBP-spezifische Th2 Zellen hatten ein größeres protektives Potential als MBP-spezifische Th1 Zellen. Die nicht ZNS-spezifischen Th1 und Th2 Zellen benötigten ihr Antigen (OVA-Peptid), um signifikant protektiv zu wirken. Durch eine Superstimulation der OVA- und MBP-spezifischen T Zellen wurde eine Neuroprotektion auf gleichem Niveau erreicht. Die Neuroprotektion nach primärer Schädigung von ZNS Gewebe ist somit antigen- und stimulationsabhängig und wird hauptsächlich von Th2 Zellen unterstützt.<br>The invasion of T cells into the central nervous system (CNS) is a hallmark of neuro inflammatory diseases like multiple sclerosis (MS) and its rodent model, experimental autoimmune encephalomyelitis (EAE), leading to activation of intrinsic macrophages, the microglia, axonal damage and break down of the blood brain barrier. The initial invading T cells are of the Th1 subtype and specific for parts of the myelin sheet like myelin basic protein (MBP). They produce inflammatory cytokines and recruit peripheral non-specific T cells and macrophages. Because these T cells are directed against a self antigen, they are called auto reactive T cells and the phenomenon an autoimmune disease. In the first part of my study I investigated the influence of auto reactive T cells on microglial cells' utilizing an organotypic slice culture system of hippocampus and entorhinal cortex. The slice culture contains a myelinated fibre tract - the tractus perforans - with its original and target neurons. Low activated MBP-specific T cells induced the expression of the activation markers ICAM-1 and MHC-II on microglia as well as microglial phagocytosis in the same manner as highly activated non-specific T cells. Only Th1 cells were able to activate microglia, while Th2 cells reduced the Th1 induced activation (ICAM-1 expression). MBP-specific Th1 cells could modulate the expression of co-stimulatory molecules B7-1 and B7-2, whereas MBP-specific Th2 cells could not. These findings could show why Th1 cells are responsible for EAE induction while Th2 cells can be protective. Auto reactive T cells like MBP-specific T cells have been found in the normal human and murine T cell repertoire. The physiological function of these cells is still unclear. Studies using the models of optic nerve crush or spinal cord crush have shown that macrophages and auto reactive T cells are involved in reorganisation and regeneration after CNS trauma. These auto reactive T cells, which are usually known to be destructive, could prevent CNS tissue from secondary degeneration. In the second part of my study I tried to identify the mechanisms involved in this phenomenon. I also used the organotypic slice culture system. Immediately after preparation causing the primary injury the slices were cultivated with T cells. Th2 cells were found to be more potent to prevent form secondary damage than Th1 cells. The non-CNS specific OVA Th1 and Th2 cells required their antigen to be fully protective. When over stimulated, MBP- and OVA-specific Th1 and Th2 cells proved to be protective to the same extend. Neuroprotection after primary injury depends on the T cell s state of activation and their antigen specificity. Among the cells examined I found Th2 cells were most effective in preventing CNS tissue from secondary injury.
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48

Ashour, DiyaaEldin [Verfasser], and Manfred [Gutachter] Lutz. "Kinetics and timing of IL-12 production by dendritic cells for Th1 polarization \(in\) \(vivo\) / DiyaaEldin Ashour ; Gutachter: Manfred Lutz." Würzburg : Universität Würzburg, 2020. http://d-nb.info/1206879327/34.

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49

Claireaux, Mathieu. "Analyses phénotypique et fonctionnelle des cellules T CD4+ spécifiques du VIH chez les patients contrôlant spontanément l’infection à VIH." Thesis, Sorbonne Paris Cité, 2017. http://www.theses.fr/2017USPCC264/document.

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Les Contrôleurs du VIH sont de rares individus capables de contrôler spontanément la réplication virale en l’absence de traitement. De nombreuses études montrent que les Contrôleurs développent des réponses T antivirales remarquablement efficaces. Les cellules T CD4+ spécifiques de Gag pourraient jouer un rôle particulier car cette population est préservée en comparaison aux patients traités et corrèle négativement avec la charge virale. Afin d’étudier cette population, nous avons réalisé une analyse transcriptionnelle et protéique multiplexée sur cellule unique, à partir de cellules T CD4+ détectées ex vivo par marquage tétramère de CMH-II contre le peptide Gag293 (Tet+). Nous avons comparé l’expression de 44 gènes et 6 protéines membranaires chez 9 patients Contrôleurs et 9 patients traités. Nous avons d’une part validé la forte fréquence de cellules T CD4+ Tet+ chez les Contrôleurs en comparaison aux patients traités et, d’autre part, montré que les cellules T CD4+ Tet+ des Contrôleurs, étaient activées et engagées dans une différenciation Th1 avancée et présentant un profil cytotoxique. De plus, les cellules T CD4+ Tet+ de Contrôleurs ont montré un état d’épuisement limité, reflété par une expression faible de PD-1, qui pourrait être l’une des raisons du maintien de leur fréquence et de leurs fonctions. Dans une deuxième étude, nous avons étudié les cellules T folliculaires « helper » (Tfh) dans la population T CD4+ spécifique de Gag chez les Contrôleurs du VIH. Les Tfh jouent un rôle essentiel dans la maturation d’affinité des anticorps en aidant les cellules B. Afin de déterminer si ce sous-type cellulaire joue un rôle dans le contrôle de l’infection à VIH, nous avons analysé le phénotype et la fonction des Tfh circulantes (cTfh) : cellules T CD4+ CD45RA- CXCR5+). Nous avons utilisé un marquage tétramère de CMH-II contre le peptide Gag293, pour détecter les cTfh spécifiques du VIH (cTfh Tet+), et nous avons montré que cette population est préférentiellement maintenue chez les Contrôleurs du VIH. L’analyse phénotypique de la population cTfh Tet+ a montré une intensité d’expression (MFI) de PD-1 plus importante dans le groupe de patients traités, suggérant une activation immune anormale chez ces patients. La fonction des cTfh, analysée pour leur capacité à induire la sécrétion d’IgG en coculture avec des cellules B mémoires autologues, n’a pas montré de différences majeures entre les groupes en terme de production d’IgG totales. Cependant, la production d’IgG spécifiques anti-VIH est significativement plus efficace chez les Contrôleurs, en particulier pour la réponse anti-Env qui est plus de 30 fois supérieure à celle des patients traités. Enfin, la fréquence des cTfh Tet+ a corrélé positivement avec la production d’IgG spécifiques, supportant l'idée d'un rôle important de la fonction Tfh dans la réponse humorale anti-VIH. L’ensemble de ces résultats indique que la population T CD4+ spécifique de Gag supporte chez les Contrôleurs les deux bras de la réponse immunitaire antivirale : d’une part, une réponse de type cellulaire Th1 montrant un profil cytotoxique et, d’autre part, une réponse de type humorale, reflétée par des interactions cTfh/B préservées, résultant en une réponse B mémoire vigoureuse. Le maintien de la fonction et de la fréquence de ces cellules spécifiques de Gag pourrait donc jouer un rôle important dans le contrôle du VIH<br>HIV Controllers are rare individuals able to spontaneously control viral replication in the absence of treatment. Several studies showed that controllers develop effective anti-viral T cell responses. Gag-specific CD4+ T cells could play a particular role in HIV control, because this population is preserved in comparison with the treated patients and correlates negatively with the viral load. In order to study this population, we performed a multiplexed single cell transcriptional and protein analysis from CD4+ T cells detected ex vivo by MHC-II tetramer labeling against the Gag293 peptide (Tet+). We compared the expression of 44 genes and 6 surface proteins in 9 Controllers patients and 9 treated patients. Firstly, we validated the high frequency of Tet+ CD4+ T cells in controllers compared to the treated patients, then we showed that Tet+ CD4+ T cells from controllers were activated and engaged in advanced Th1 differentiation with a cytotoxic profile. In addition, Tet+ CD4+ T cells from controllers showed a limited state of exhaustion, reflected by a lower expression of PD-1, which could be one of the reasons for maintaining their frequency and functions. In a second study, we studied follicular helper T cells (Tfh) among the Gag-specific CD4+ T cell population of HIV controllers. Tfh plays an essential role in the affinity maturation of the antibody response by providing help to B cells. To determine whether this CD4+ T cell subset may contribute to the spontaneous control of HIV infection, we analyzed the phenotype and function of circulating Tfh (cTfh: T cells CD4+ CD45RA- CXCR5+). We performed a MHC-II tetramer labeling against Gag293 peptide to detect HIV-specific cTfh (cTfh Tet +), and showed that this population is preferentially maintained in HIV controllers. Phenotypic analysis of Tet+ cTfh population showed a higher intensity of PD-1 expression (MFI) in the treated group suggesting abnormal immune activation in these patients. The function of cTfh, analyzed by the capacity to promote IgG secretion in cocultures with autologous memory B cells, did not show major differences between groups in terms of total IgG production. However, the production of HIV-specific IgG is significantly more efficient in the controller group, especially for the anti-Env response that is more than 30-fold greater than those of the treated patients. Finally, the frequency of Tet+ cTfh correlated positively with the production of specific IgG, supporting the idea of an important role of Tfh function in the humoral antiHIV response. Taken together, these results indicate that Gag-specific CD4+ T cell population supports the two arms of the antiviral immune response in HIV controllers: the cell-mediated response through a preferential differentiation toward Th1 cell type showing a cytotoxic profile, and the humoral response, reflected by preserved cTfh / B interactions, resulting in a vigorous memory response. Maintaining the function and frequency of these Gag-specific CD4+ T cells could therefore play an important role in HIV control
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Lucas, Casaca Vera Isabel [Verfasser], and Bianca [Akademischer Betreuer] Schaub. "Role of Th1 and Th2 cell-specific polymorphisms and of Regulatory T cells modulated by farm exposure for the determination of childhood allergic diseases / Vera Isabel Lucas Casaca. Betreuer: Bianca Schaub." München : Universitätsbibliothek der Ludwig-Maximilians-Universität, 2014. http://d-nb.info/1055907637/34.

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