Análise da capacidade migratória e da ativação de linfócitos T CD4+ por células dendríticas na paracoccidioidomicose expeimental / Analysis of the capacity of migration and activation of TCD4+ lymphocytes by dendritic cells in experimental paracoccidioidomycosis

Santos, Suelen Silvana dos

19 August 2010

Paracoccidioidomicose (PCM) é uma micose sistêmica causada por Paracoccidioides brasiliensis (P. brasiliensis), que acomete preferencialmente o pulmão, sendo este um dos poucos órgãos que está em continua e intensa interação com o meio ambiente e o sistema imune. O grande desafio para o sistema imune pulmonar é discriminar o que é nocivo e reagir de acordo. As células dendríticas (DCs) são apresentadoras de antígenos \"profissionais\" capazes de fazer o processamento do antígeno e a apresentação de peptídeos a linfócitos T e são ideais para manter este equilíbrio delicado entre a tolerância e uma resposta imune efetora. Sabendo da importância dessas células no sistema imune e que a infecção por P. brasiliensis ataca preferencialmente o pulmão, células de lavado broncoalveolar (BAL), após infecção experimental com leveduras de P. Brasiliensis, foram analisadas. Nós observamos um significante aumento de DCs no BAL após 24hrs da infecção intratraqueal com 104 leveduras de P. brasiliensis. A caracterização das DCs mostraram que essas células expressaram CD11c, MHC-II e DEC205. A fim de verificar a capacidade de migração das DCs, as mesmas foram diferenciadas a partir de células de medula óssea e pulsadas com leveduras de P. brasiliensis, marcadas com CFSE e injetadas intratraquealmente em camundongos. Como controle negativo, utilizamos PBS e DCs não pulsadas com o fungo. Os resultados mostraram, que após 12 horas de infecção, as DCs (CFSE+CD11c+), migraram para os linfonodos torácicos. No entanto, a quantidade destas células diminui discretamente após 24 horas de infecção. Além disso, não observamos DCs nos linfonodos regionais, quando analisamos os grupos controle. Dessa forma, as células pulmonares também foram marcadas in vivo injetando-se intratraquealmente o corante CFSE juntamente com leveduras de P. brasiliensis. Verificamos que após 12 horas, as DCs pulmonares, dos animais infectados com o fungo, migraram para os linfonodos regionais. Esses resultados comprovam que o fungo P. brasiliensis foi capaz de ativar as DCs, induzindo sua migração para linfonodos regionais, e induziu nesse órgão uma resposta por células T evidenciada pela produção preferencial de IL-10. / Paracoccidioidomycosis (PCM) is a systemic mycosis caused by Paracoccidioides brasiliensis (P. brasiliensis), which mainly affects the lungs. They are one of the few organs that are in constant and intense interaction with the environment and the immune system. The great challenge for the pulmonary immune system is to discriminate what is harmful and react accordingly. Dendritic cells (DCs) are \"professionals\" antigen-presenting cells and they can do the antigen processing. They can also do the presentation of peptides to T lymphocytes and are ideal for maintaining this delicate balance between tolerance and an effector immune response. Knowing the importance of these cells in the immune system and that the infection by P. brasiliensis preferentially attacks the lungs, cells from bronchoalveolar lavage (BAL), after experimental infection with yeasts of P. Brasiliensis, were analyzed. We observed a significant increase of DCs in BAL after 24 hours of intratracheal infection with 104 of yeast cells of P. brasiliensis. The characterization of these cells showed that DCs expressed CD11c, MHC-II and DEC205. In order to verify the ability of migration of DCs, they were differentiated from bone marrow cells and pulsed with yeasts of P. brasiliensis, they were also labeled with CFSE and injected intratracheally into mice. As a negative control, we used PBS and DCs that were not pulsed with the fungus. The results showed that after 12 hours of infection, the DCs (CFSE + CD11c +), migrated to the thoracic lymph nodes. However, the quantity of these cells decreases slightly after 24 hours of infection. Furthermore, we observed no DCs in regional lymph nodes when we analyzed the control groups. Thus, the lung cells were also labeled in vivo by injecting the CFSE dye intratracheally with yeasts of P. brasiliensis. We found that after 12 hours, pulmonary DCs of the animals infected with the fungus migrated to regional lymph nodes. These results indicate that the fungus P. brasiliensis was able to activate DCs, inducing their migration to regional lymph nodes, and inducing a response in that organ by T cells as evidenced by preferential production of IL-10.

Células dendríticas

Dendritic cells

Paracoccidioides brasiliensis

Paracoccidioides brasiliensis

Paracoccidioidomicose

Paracoccidioidomycosis

Efeitos do estresse agudo de contenção sobre a caracterização fenotípica e funcional de células dendríticas em camundongos Balb/c / Effects of acute restraint stress on phenotypic and functional characterization of dendritic cells in Balb/c mice

Lima, Ana Paula Nascimento de

14 March 2014

Os efeitos do estresse, que são fatores constantes e componentes importantes na vida de um indivíduo, provocam alterações sobre o sistema imunológico. Nossa hipótese foi de que o estresse agudo de contenção aplicado em três sessões em dias alternados pode alterar a expressão de marcadores de membrana e a função de células dendríticas (DCs) de camundongos Balb/c. Investigar os efeitos do estresse sobre as DC nos pareceu relevante uma vez que estas são importantes elementos de ligação entre as respostas imune inata e adaptativa, ou seja, são células apresentadoras de antígenos altamente especializadas com uma capacidade única para ativar linfócitos T. Inicialmente, foram realizados experimentos comportamentais e dosagens de hormônios relacionados à resposta ao estresse, a fim de caracterizar e validar o modelo de estresse agudo por contenção utilizado. Em seguida, DCs esplênicas e DCs geradas a partir de células precursoras da medula óssea foram analisadas quanto a expressão de marcadores fenotípicos CD11c, MHC-II, CD80, CD86, CD40 e CCR-7. O modelo de estresse agudo de contenção mostrou-se capaz de produzir alterações no comportamento e de ativar o eixo HPA e o SNS. A análise dos marcadores fenotípicos revelou um aumento da expressão de CD40 em DCs esplênicas de animais estressados, porém, não houve alterações nas DCs derivadas da medula óssea. O ensaio de proliferação demonstrou uma alteração na função de DCs na proporção de 1:1 no co-cultivo com esplenócitos. O presente trabalho, portanto, demonstrou que o estresse agudo de contenção, realizado em três sessões em dias alternados, é capaz de alterar alguns parâmetros relacionados ao fenótipo e à função de DCs esplênicas. / The effects of stress which are constant factors and important components in an individual\'s life cause changes on the immune system. Our hypothesis was acute restraint stress in three sessions on alternate days can change the expression of membrane markers and the function of dendritic cells (DCs) in BALB/c mice. Evaluate the effects of stress on the DC seemed to be relevant since these are important elements linking innate and adaptive immune responses, i,e., cells are highly specialized antigen-presenting with a unique capacity to activate T cells. First of all, behavioral assessment and dosages of hormones related to stress response were conducted to characterize and to validate the model of acute restraint stress. Then, splenic DCs and DCs generated from bone marrow were analyzed for expression of phenotypic markers CD11c, MHC-II, CD80, CD86, CD40 and CCR-7. The model of acute restraint stress changed the behavior and activate the HPA axis and the SNS. The analysis of phenotypic markers revealed an increased expression of CD40 on splenic DCs from stressed animals, however, there were no changes in BM-dDCs. The proliferation assay showed a change in the function of DCs in the coculture with splenocytes in a ratio of 1:1. Therefore, the present study indicated that acute restraint stress, conducted in three sessions on alternate days, is able to change some parameters related to the phenotype and function of splenic DCs.

Células dendríticas

Dendritic cells

Estresse

Neuimmunomodulation

Neuroimunomodulação

Stress

Caracterização fenotípica de células dendríticas transfectadas com scFv obtido a partir de anticorpo monoclonal anti-idiotípico Ab2-β, que mimetiza o antígeno gp43 de Paracoccidioides brasiliensis / Phenotypic characterization of dendritic cells transfected with scFv derived from monoclonal anti-β-idiotypic Ab2 which mimics the antigen gp43 of Paracoccidioides brasiliensis

Jannuzzi, Grasielle Pereira

24 September 2013

A paracoccidioidomicose (PCM) é um a micose profunda de natureza granulomatosa, causada pelo fungo Paracoccidioides brasiliensis (P. brasiliensis) e que compromete preferencialmente o tecido pulmonar. O P. brasiliensis sintetiza várias substâncias, dentre estas, destaca-se a glicoproteína de 43 kDa (gp43), a qual é considerada o principal componente antigênico do fungo. Dada a importância da gp43, anticorpos monoclonais (Mabs) contra esta glicoproteína foram obtidos e posteriormente caracterizados. Baseado na hipótese da rede idiotípica, Jerne (1974) propôs que cada anticorpo, quando produzido em resposta a um antígeno, induz a formação de outros anticorpos dirigidos contra sua região variável, na qual é única. Anticorpos anti-idiotípicos, que reconhecem o paratopo, contendo a imagem interna do antígeno, são denominados de Ab2-β e seu potencial terapêutico tem sido explorado em diferentes sistemas. Apesar da molécula de anticorpo ser complexa estruturalmente, sabemos que a região Fab, é a responsável pelo mimetismo do antígeno. Então, nosso grupo de pesquisa construiu uma nova molécula de anticorpo à partir do Mab anti-idiotípico Ab2-β, que mimetiza o antígeno gp43 de P. brasiliensis, denominada de fragmento variável de cadeia única (scFv). A transfecção dessa molécula em células dendríticas (DCs) mostrou ser promissora na PCM experimental, visto que estes transfectomas foram eficientes em apresentar a proteína scFv às células dos linfonodos, induzindo linfoproliferação, além de diminuírem a carga fúngica pulmonar. Visto que a molécula de scFv que possui a região de reconhecimento e ativação de linfócitos T mostrou eficiência no modelo de terapia na PCM experimental, o principal objetivo deste trabalho foi analisar os mecanismos pelos quais os transfectomas de DCs ativam a resposta imune em camundongos infectados com o fungo, para que possamos entender melhor a capacidade destas células em modular a resposta imune na PCM experimental. Dessa maneira, avaliamos a capacidade das DCs trasfectadas com pMAC/PS-scFv em migrar para os linfonodos regionais e induzirem uma resposta protetora com produção de IgG, bem como, analisamos o fenótipo destas células e produção de citocinas. Nosso modelo de terapia com pMAC/PS-scFv mostrou-se eficiente, uma vez que observamos diminuição de células T regulatórias nos linfonodos regionais, bem como aumento da produção de citocinas como IFN-γ e IL-12. Ainda, observamos aumento do isotipo IgG2b, sugerindo a modulação de resposta imune para o tipo Th1, importante na proteção da PCM. / The paracoccidioidomycosis (PCM) is the nature of granulomatous mycosis caused by Paracoccidioides brasiliensis (P. brasiliensis) and preferentially compromises lung tissue. The P. brasiliensis synthesizes various substances, among these, there is a 43 kDa glycoprotein (gp43), which is considered a major antigenic component of the fungus. Given the importance of gp43 monoclonal antibodies (Mabs) against this glycoprotein were obtained and further characterized. Based on the idiotypic network hypothesis, Jerne (1974) proposed that each antibody, when produced in response to an antigen, induces the several of other antibodies production against its variable region, which is unique. Anti-idiotypic antibodies that recognize the paratope containing the internal image of the antigen are called Ab2 β and their therapeutic potential has been explored in different systems. Although the antibody molecule is structurally complex, we know that the Fab region, is responsible for antigen mimicking. Therefore, our research group has engineered a new molecule from the antibody Mab-anti-idiotypic Ab2 β that mimics the antigen gp43 of P. brasiliensis, known as single chain variable fragment (scFv). Transfection of this molecule on dendritic cells (DCs) has shown promise in experimental PCM, since these transfection were effective scFv protein present in the cells of the lymph nodes, inducing lymphoproliferation, in addition to reducing fungal burden in the lung. Since the scFv molecule that has the region recognition and activation of T lymphocytes showed efficiency in therapy model in experimental PCM, the main objective of this study was to analyze the mechanisms by which transfected DCs activate the immune response in infected mice with the fungus, so that we can better understand the ability of these cells to modulate the immune response in experimental PCM. Thus, the capacity of transfected DCs with pMAC / PS-scFv to migrate to regional lymph nodes and induce a protective response with IgG production, as well as analyze the phenotype of these cells and cytokine production. Our therapy model with pMAC / PS-scFv was efficient, since we observed decrease of regulatory T cells in regional lymph nodes, as well as increased production of cytokines such as IFN-γ and IL-12. Furthermore, we observed increased IgG2b isotype, suggesting modulation of the immune response to a Th1 response, the protect model of experimental PCM.

Células dendríticas

Dendritic cells

Paracoccidioidomicose

Paracoccidioidomycosis

scFv

scFv

Caracterização fenotípica e funcional de células dendríticas após vagotomia unilateral cervical em camundongos C57BL/6 / Phenotypic and functional characterization of dendritic cells following unilateral cervical vagotomy in C57BL/6 mice

Cruz, Daniel Sanzio Gimenes da

04 July 2013

O nervo vago exerce um papel importante na regulação da homeostase, e seus ramos eferentes emitem sinais capazes de atenuar a resposta inflamatória através da via do reflexo inflamatório. Nossa hipótese foi de que esta via pode também alterar a função das células dendríticas (DCs), uma vez que estas células possuem receptores colinérgicos e podem ser reguladas pelas citocinas inflamatórias. Sendo assim, DCs esplênicas e DCs geradas a partir de células precursoras da medula óssea de animais vagotomizados unilateralmente foram analisadas quanto aos marcadores fenotípicos CD11c e MHC-II e as moléculas co-estimuladoras CD80 e CD86. As DCs derivadas da medula óssea ainda foram avaliadas quanto a função fagocítica, a apresentação de antígenos, bem como, a produção de citocinas do cocultivo destas com linfócitos de camundongos OT-II. Um ensaio de reação de hiperensibilidade tardia (DTH) para se avaliar a resposta imune celular também foi realizado, mas não mostrou alterações significantes. A análise dos marcadores fenotípicos revelou um aumento da expressão de CD80 em DCs esplênicas de animais vagotomizados unilateralmente, mas não houveram alterações nas DCs derivadas da medula óssea. A avaliação da capacidade fagocítica revelou uma diminuição significante em DCs derivadas da medula óssea de animais vagotomizados unilateralmente enquanto no ensaio de proliferação de linfócitos OTII não houve efeito significante. Entre as citocinas avaliadas, a IL-6 e IFN-ϒ se apresentaram aumentadas nos animais vagotomizados unilateralmente. Portanto, o presente trabalho foi capaz de evidenciar que as DCs também estão sujeitas à modulação do sistema nervoso parassimpático, e que, uma vez moduladas, estas células são capazes de exercer influências sobre outras células do sistema imunológico. / The vagus nerve plays an important role in the regulation of homeostasis and its efferent branches emit signals capable of attenuating the inflammatory response via the inflammatory reflex. Our hypothesis was that this pathway may also alter the function of dendritic cells (DCs), since these cells have cholinergic receptors and can be regulated by the inflammatory cytokines. Thus, splenic DCs and DCs generated from bone marrow precursor cells unilaterally vagotomized animals were analyzed for phenotypic markers CD11c and MHC-II and co-stimulatory molecules CD80 and CD86. The bone marrow-derived DCs were also evaluated for phagocytic function, antigen presentation, as well as the production of cytokines such co-culture with lymphocytes from mice OT-II. A delayed type hypersensitivity test (DTH) twas also performed to evaluate the cellular immune response was also performed, but showed no significant changes. The analysis of phenotypic markers showed increased CD80 expression in splenic DCs from unilaterally vagotomized animals but there were no changes in bone marrow-derived DCs. The evaluation of phagocytic ability showed a significant decrease in DCs from unilaterally vagotomized animals while in the OT-II lymphocyte proliferation assay there was no significant effect. Among the cytokines evaluated, IL-6 and IFN-ϒ were increased in unilaterally vagotomized animals. Therefore, this study was able to demonstrate that DCs are also subject to modulation of the parasympathetic nervous system, which, once modulated, these cells are able to exert influence on other cells.

células dendríticas

dendritic cells

nervo vago

neuroimmunomodulation

neuroimunomodulação

vagus nerve

O papel da heme oxigenase-1 na modulação de células dendríticas levando à proteção da lesão por isquemia e reperfusão. / The role of heme oxygenase-1 in dendritic cells modulation leading to ischemia and reperfusion injury protection.

Amano, Mariane Tami

26 September 2011

A isquemia e reperfusão (IR) é a principal causa de insuficiência renal aguda. Evidências mostram a participação de linfócitos T e células dendríticas (DC) na lesão por IR. Entretanto, os mecanismos envolvidos não estão claros. A enzima heme oxigenase (HO)-1 está relacionada à diminuição de respostas inflamatórias. Neste trabalho, investigamos a participação de linfócitos T CD4+ e DC na proteção da lesão por IR induzida pela HO-1. Injetamos em camundongos um indutor de HO-1 (Hemin), e realizamos a IR. Avaliamos a lesão pela uréia e creatinina no soro, a expressão de citocinas por RT-PCR, nível de proteínas por bioplex e perfil celular por FACS. Observamos que a HO-1 protegeu da lesão por IR. A diminuição de INFg com a HO-1 sugeriu uma menor ativação de linfócitos T. No entanto, a transferência de células CD4+ tratadas com Hemin não apresentou diferença. Vimos que a HO-1 alterou o fenótipo das DC após IR e suprimiu a produção de TNFa pelas mesmas. Concluímos que a proteção pela HO-1 é capaz de modular a resposta inflamatória de DC, diminuindo o TNFa. / The ischemia and reperfusion (IR) is the main acute kidney injury. Evidences have shown the role of CD4+ T cells and dendritic cells (DC) in the IR injury. However, the mechanisms involved in the participation of these cells are not clear. The heme oxygenase (HO)-1 enzyme is associated to decrease in inflammatory responses. In this work, we investigated the role of CD4+ T cells and DC in renal injury protection induced by HO-1. We injected in mice a HO-1 inducer (Hemin), and we did the IR. Renal injury was evaluated by serum levels of urea and creatinine, cytokines expression by RT-PCR, proteins level by bioplex and cell profile by FACS. We observed that HO-1 lead to IR injury protection. The IFNg decrease with HO-1 suggested less T cells activation. However, transfer of hemin treated CD4+ cells did not differ from the other group. We observed that HO-1 altered DC phenotype after IR and suppressed TNFa production by these cells. We concluded that the protection by HO-1is able to modulate DC inflammatory response, diminishing TNFa.

Células dendríticas

Dendritic cells

Ischemia

Isquemia

Kidney

Linfócitos

Lymphocytes

Rim

Regulation of E Protein Activity During Dendritic Cell Development

Grajkowska, Lucja Teresa

January 2015

Dendritic cells are a key population in the immune system. There are two main subsets: conventional DC (sometimes called classical DC, cDCs), which survey tissues for pathogens and activate naive T cells, and plasmacytoid dendritic cells (pDCs), which produce high amounts of IFNα in response to viral products. Both subsets begin development in the bone marrow from common dendritic progenitor (CDP), and driven by Flt3 signaling induced by the growth factor Flt3L. The CDP gives rise to a cDC committed preDC which exits the bone marrow and seeds peripheral organs to give rise to cDCs, while pDCs finish development in the bone marrow and migrate into the periphery as mature cells. pDC development is directed by E2-2, a member of the E protein family of basic helix-loop-helix transcription factors that are obligate dimers and bind an E-box sequence. E proteins are antagonized by Id proteins, and Id family member Id2 is required for cDC development. The apparently cell intrinsic choice of pDC vs. cDC fate is determined by the net activity of E proteins. Loss of E2-2 affects only pDC development, but its expression is not as specific, as E2-2 is also expressed in cDCs, macrophages and B cells. E2-2 expression in cDCs was particularly puzzling, considering the dependence of cDCs on Id2, the E2-2 antagonist. We strived to address the discrepancy between the very specific activity of E2-2 in pDC development and its broader expression. This work shows that the E2-2 locus encodes two independently regulated isoforms. E2-2Long, the more active isoform is expressed only in pDCs, and E2-2Short, the less transcriptionally active isoform, is expressed more broadly. Moreover, E2-2Long is required for optimal pDC development. Homozygous loss of just E2-2Long leads to lower pDC frequency in the spleen and phenotypically affected pDCs in the periphery. Although E2-2 is essential for pDC development, no signal has yet been identified that induces E2-2 expression to influence pDC over cDC fate. Given the essential nature of E2-2 in pDC development, we aimed to understand better how E2-2 is regulated during pDC fate specification. We examined an E2-2Long reporter and found that E2-2Long expression precedes pDC commitment in early progenitors. E2-2 is only upregulated in committed pDCs, and actively shut down in cDCs through the expression of Id2. Analysis of E2-2 in an in vitro time controlled model of dendritic cell development showed that all dendritic cells (both cDCs and pDC) go through an E2-2 expressing stage only to resolve into E2-2- cDCs and E2-2+ pDCs. Early E2-2 expression and E2-2 upregulation upon pDC commitment hinted at the presence of an E2-2 controlled cis-regulatory module. ChIP-Seq data showed only one peak of E2-2 binding located 150 kb downstream of the TCF4 gene. Heterozygous deletion of this region in the in vitro DC development model led to impaired pDC development and a fail to undergo the E2-2+ stage described above. The regulatory element is essential for E2-2 upregulation during DC development. This work describes two new mechanisms of E protein regulation during dendritic cell development: cell specific differential isoform usage and a distal cis regulatory element responsible for enforcing and upregulating E2-2 expression. These new mechanisms can lead to better understanding of how this family of broadly expressed and pleiotropic transcription factors is regulated, with implications in overall development, not only dendritic cell fate decision.

Proteins--Synthesis--Regulation

Molecular immunology

Dendritic cells

Immunology

Genetics

Delineating Human Dendritic Cell Development

Lee, Jaeyop

January 2016

The origin of human dendritic cells (DCs) has long been debated. DCs are a subset of innate immune cells that are essential for initiating adaptive immune responses. Determining their ontogeny is critical for vaccine development and for unveiling the molecular mechanism of DC insufficiency, which underlies many primary immune deficiency disorders and leukemia. Like all blood cells, human DCs develop from hematopoietic stem cells through a sequence of increasingly restricted progenitors. Initially it was assumed that DCs should derive exclusively from myeloid progenitors. However, during the past few decades, a number of myeloid and lymphoid progenitors have been described and shown to have DC potential, instigating the debate of the myeloid vs. lymphoid origin of DCs. Hindering the resolution of this debate, human DC-restricted progenitors had not been identified. Further, the potential of known progenitors could not be interrogated due to the lack of a culture system that supports simultaneous differentiation of all human DCs subsets, in conjunction with other myeloid and lymphoid cells. In this work, we establish a culture system that supports the development of the three major subsets of DCs (plasmacytoid DCs or pDCs, and the two classical DCs, cDCs) as well as granulocytes, monocytes and lymphocytes. This system combines mitomycin C-treated murine stromal cell lines, MS5 and OP9, together with human recombinant cytokines, FLT3L, SCF and GM-CSF, and supports the differentiation of progenitor cells at a population and single cell level. Using this culture in combination with a phenotypic characterization of CD34+ progenitor cells, we identify four consecutive DC progenitors with increasing degree of commitment to DCs and describe their anatomical location of development. We show that DCs develop from a granulocyte-monocyte-DC progenitor (GMDP), which produces granulocytes and a monocyte-DC progenitor (MDP), which then generates monocytes and a common DC progenitor (CDP), which produces pDCs and a cDC precursor (pre-cDC), which finally produces cDCs only. Lastly, we establish a staining panel that allows the phenotypic identification and separation of newly found DC progenitors as well as all previously described myeloid and lymphoid progenitors. We investigate their inter-developmental relationship and DC potential at the single cell level. We show that each progenitor population with homogeneous phenotype is heterogeneous in developmental potential and prove that cell surface marker expression cannot be directly equated to a specific developmental potential. In order to resolve the unreliability of phenotype to draw developmental pathways, we propose to use the quantitative clonal output in order to delineate the DC developmental pathway. In summary, our studies provide a new tool to determine DC potential in vitro, identify new stages of DC development, and propose a new method for tracing the developmental pathway for DC lineage. This will generate a new model of dendritic cell hematopoiesis that can explain and reconcile the conflicts of data on DC origin and development.

Immune response

Hematopoiesis

Cells--Growth

Dendritic cells

Immunology

Oncology

Medicine

Investigating regulation of immune responses during Trichuris muris infection

Klementowicz, Joanna

January 2012

Infection with human gastrointestinal (GI) parasites, such as Trichuris trichiura, affects more than billion people worldwide, causing significant morbidity and health problems especially in poverty-stricken developing countries. Despite extensive research, the mechanisms of induction and regulation of effector immune responses against these parasites are incompletely understood, which hinders the development of anti-parasite therapies. Infection with GI parasite is usually chronic suggesting that parasites are capable of modulating immune responses of their host to prevent expulsion. However, mechanisms by which parasites control host immunity to allow infection are still ill-defined. The aim of this PhD study was to characterise the role of different immunoregulatory mechanisms in immunity to GI parasite infection, with a focus on dendritic cells (DCs), regulatory T cells (Tregs) and the regulatory cytokine transforming growth factor β (TGF-β).Here we showed for the first time that loss of TGF-β-activating integrin alphavβ8 specifically on DCs resulted in protection from chronic infection with Trichuris muris, a mouse model of T. trichiura infection in man. Accelerated expulsion was immune-mediated and although increased levels of protective Th2 cytokines were observed very early during infection, elevated levels of non-protective Th1 cytokines were also detected. Partial depletion of CD4+ or FcεRI+ cells had no effect on the observed phenotype. Since deletion of alphavβ8 on DCs results in decreased numbers of Tregs in the gut, we tested whether depletion of Tregs using a mouse model that allows conditional ablation of Foxp3+ Tregs (DEREG mice) would alter infection development. Although transient Treg depletion at the beginning of infection had no major effect on expulsion kinetics, we observed a tendency for enhanced Th2 responses in DEREG mice. Moreover, even though DC-mediated TGF-β activation via alphavβ8 integrin was essential for T. muris infection development, transient depletion of DCs had no effect on the induction of Th2 responses or parasite expulsion. These data indicate a novel role for the TGF-β-activating integrin alphavβ8 and DCs in regulating effector immune responses during T. muris infection and may contribute to the development of new anti-parasite therapies.

Control of Th2 polarisation by dendritic cells and natural killer cells

Walwyn-Brown, Katherine

January 2018

Type 2 (Th2) immune responses are required for immune defence against helminths, but can also have pathogenic effects in allergic conditions. This thesis examined two factors which may influence Th2 immunity at a cellular and molecular level: cross-talk between Natural Killer (NK) cells and dendritic cells (DCs) and the cell surface organisation of DCs. Cross-talk between NK cells and DCs is well-established to impact Th1 responses against tumours and infection; however the influence of this interaction during Th2 inflammation is unknown. To investigate this, human monocyte-derived DCs were stimulated in vitro with different pathogen-associated molecules; LPS or Poly(I:C) which polarise a Th1 response, or soluble egg antigen (SEA) from the helminth worm Schistosoma mansoni, a potent Th2-inducing antigen. These cells were then combined with autologous NK cells. Confocal microscopy showed polarisation of the NK cell microtubule organising centre (MTOC) and accumulation of LFA-1 at contacts between NK cells and immature or Th2-polarising DCs, but not Th1-polarising DCs, indicative of the assembly of an activating immune synapse. NK cells did not lyse DCs treated with LPS or Poly(I:C), but degranulated to and lysed both immature DCs and Th2 polarising DCs. Antibody blockade of NK cell activating receptors NKp30 and DNAM-1 prevented this lysis. Furthermore, depletion of NK cells in mice which were then transferred with Th2 polarising DCs led to an enhanced Th2 recall response. Thus, these data indicate a previously unrecognised role of NK cell cytotoxicity in restricting the pool of DCs involved in Th2 immune responses. Secondly, this thesis investigated the nanoscale organisation of MHC-II on the surface of Th1 and Th2 polarising DCs using ground state depletion super-resolution microscopy. MHC-II was relatively homogenously distributed across the membrane with no significant changes in clustering between immature, Th1 and Th2 polarising DCs. In contrast, imaging CD74, which can mediate internalisation of MHC-II, revealed increased expression and a more homogenous distribution of this receptor on the surface of Th2-polarising DCs compared to Th1-polarising DCs. These data suggest that changes in the clustering of CD74 could modulate MHC-II surface expression during Th2 responses. Overall, the results in this thesis indicate that both molecular and cellular level modulation of DC function contribute to the development of Th2 responses.

Influência da deformação plástica no tratamento térmico de homogeneização de um aço ferramenta para trabalho a frio / Influence of plastic deformation at homogenization heat treatment of a cold work tool steel

Xavier, Rodrigo Yokoyama [UNESP]

30 January 2017

Submitted by RODRIGO YOKOYAMA XAVIER null (rodyok@hotmail.com) on 2017-02-16T01:10:07Z No. of bitstreams: 1 Dissertação Mestrado - Rodrigo Yokoyama Xavier.pdf: 6767206 bytes, checksum: 36a0ac2db721a2114f623ea26fe9f582 (MD5) / Approved for entry into archive by Juliano Benedito Ferreira (julianoferreira@reitoria.unesp.br) on 2017-02-22T17:27:06Z (GMT) No. of bitstreams: 1 xavier_ry_me_guara.pdf: 6767206 bytes, checksum: 36a0ac2db721a2114f623ea26fe9f582 (MD5) / Made available in DSpace on 2017-02-22T17:27:06Z (GMT). No. of bitstreams: 1 xavier_ry_me_guara.pdf: 6767206 bytes, checksum: 36a0ac2db721a2114f623ea26fe9f582 (MD5) Previous issue date: 2017-01-30 / O nível de qualidade de peças produzidas a partir de grandes lingotes está intimamente relacionado à qualidade dos lingotes em si. Dentre os diversos defeitos inerentes ao processo de solidificação, destacam-se as microssegregações de elementos de liga, que causam uma deterioração nas propriedades do produto final. Uma maneira de reduzir o dano causado pela microssegregação é através do Tratamento Térmico de Homogeneização, este por sua vez demanda elevados tempos de processo, elevando custos e tempos de fabricação. Uma das formas de reduzir os tempos de homogeneização, uma vez que este apresenta caráter difusional, é através da redução do espaçamento interdendrítico. Neste trabalho foi analisada a influência da deformação plástica como forma de reduzir o espaçamento entre dendritas no tratamento térmico de homogeneização. Para tal fim, utilizou-se um lingote fundido em aço ferramenta de composição química similar ao AISI A2. As amostras foram retiradas do núcleo do lingote no estado bruto de solidificação e sofreram deformações de 0,6 e 1,3 através do processo de laminação a quente, sendo temperadas em água na sequência. Após laminadas as amostras passaram por um tratamento térmico de homogeneização na temperatura de 1200°C por 8h ou 16h e foram novamente temperadas em água. As análises foram feitas através de Microscopia Óptica, Dureza Vickers, Difratometria de Raios-X e Microscopia Eletrônica de Varredura. Foi observado em todas as amostras a presença de microrechupes, e uma microestrutura composta predominantemente por dendritas oriundas da solidificação, identificadas pela fase martensítica, envoltas por uma matriz formada de austenita retida, contendo carbonetos e sulfetos. Com a deformação plástica foi possível quebrar a estrutura dendrítica a aproximar as regiões segregadas das não segregadas. O tratamento térmico por um tempo de 8h não foi suficiente para homogeneizar a microestrutura e reduzir as microssegregações, independentemente do estado de deformação das amostras. O tratamento térmico por 16h apresentou os melhores resultados em relação à homogeneidade química, sendo tanto melhor o resultado quanto maior a deformação imposta às amostras. / The quality of pieces produced from large ingots is closely related to the quality of ingots itself. Among the various defects inherent to the solidification process, there is the microsegregation of alloying elements, causing a deterioration in the properties of the final product. One way to reduce the damage caused by microsegregation is through the homogenization heat treatment, this in turn demands long time of process, increasing costs and lead-times for manufacture. One way to reduce the homogenization time, since it has a diffusive character, is by reducing the interdendritic spacing. In this study was analyzed the influence of plastic deformation as a mean to reduce the spacing between dendrites in the homogenization heat treatment. For this purpose it was used a cast ingot of chemical composition similar to the AISI A2 tool steel. Samples were cut from the ingot center in the as-cast state and suffered deformations of 0.6 and 1.3 through the hot rolling process and quenched in water in the sequence. After rolling the samples passed through a homogenization heat treatment at a temperature of 1200°C for 8h and 16h and again were quenched in water. Analyses were performed by Optical Microscopy, Vickers Hardness, X-Ray Diffractometry and Scanning Electron Microscopy. It was observed in all samples the presence of microcavities, and a microstructure consisting predominantly by solidifications dendrites identified by a martensitic phase, involved by a retained austenite matrix containing carbides and sulfides. The plastic deformation broke the dendritic structure, and approached the segregated regions to the non-segregated regions. The heat treatment for 8h was not sufficient to homogenize the microstructure and reduce the microsegregation, independently of the deformation state of the samples. The heat treatment for 16h presented the best results in relation to the chemical homogeneity, and the better the result as the greater the deformation imposed on the samples.

Solidificação

Segregação

Estrutura dendrítica

Homogeneização

Solidification

Segregation

Dendritic structure

Homogenization