Efeitos de diferentes emulsões lipídicas sobre a expressão de moléculas de superfície envolvidas no processo de apresentação de antígenos em células mononucleares humanas in vitro / Effects of different lipid emulsions on surface molecules expression involved in antigen presentation process on human mononuclear cells in vitro

Thiago Manzoni Jacintho

13 December 2004

Moléculas HLA-DR e co-estimulatórias tem papel central na função imune de leucócitos. Diferentes emulsões lipídicas (EL) podem alterar funções imunes de leucócitos. Para avaliar os efeitos de diferentes EL sobre a expressão de moléculas HLA-DR, CD80 e CD86 presentes na superfície de monócitos/macrófagos (MO/M?) e CD28 e CD152 presentes na superfície de linfócitos T auxiliares (L? CD4) humanos, células mononucleares do sangue periférico de voluntários saudáveis (n=10) foram separadas com uso de Ficoll Hypaque (d=1,007) e incubadas por 48 horas (MO/M?) e 72 horas (L?) em meio RPMI 1640 acrescidas ou não (controle negativo) de diferentes EL comerciais ou misturas experimentais na concentração de 1mg/mL. De acordo com o tipo da emulsão lipídica adicionada ao meio de cultura, as células foram divididas em seis grupos experimentais: a) Controle negativo - células mononucleares cultivadas sem o acréscimo de EL b) TCLn-6 - células mononucleares cultivadas com EL a base de óleo de soja rica em ácidos graxos poliinsaturados tipo n-6 (AGPI n-6), c) TCLn-6/TCLn-3 - células mononucleares cultivadas com mistura experimental contendo 80% da EL a base de óleo de soja e 20% de EL a base de óleo de peixe rica em AGPI tipo n-3, d) TCM/TCLn6 - células mononucleares cultivadas com EL composta por 50% óleo de coco, rico em triglicérides de cadeia média e 50% de óleo de soja, e) TCM/TCLn-3 - células mononucleares cultivadas com mistura experimental contendo 80% de EL composta por 50% óleo de coco e 50% de óleo de soja e 20% de EL a base de óleo de peixe, f) SMOF - células mononucleares cultivadas com a nova EL contendo 30% de óleo de soja, 30% de triglicérides de cadeia média, 25% de óleo de oliva e 15% de óleo de peixe. As células mononucleares foram ativadas pelo uso de 10?g/mL de fitohemaglutinina. A expressão das moléculas de superfície foi analisada por citometria de fluxo. A porcentagem de fluorescência, que indica o número de células expressando as moléculas em estudo e a intensidade de fluorescência, que indica de forma indireta o número de moléculas expressas por células, foram medidas. Os resultados obtidos foram submetidos à teste estatístico Friedman e pós-teste Student-Newman-Keuls, adotando-se nível de significância de p<0,05. Devido às diferenças na expressão basal dos doadores, os resultados de intensidade de fluorescência foram transformados em porcentagem relativa ao controle basal (Basal=100). Nos grupos TCLn-6, TCLn-6/TCLn-3, TCM/TCLn-6, TCM/TCLn-3 e SMOF, a intensidade de fluorescência de moléculas HLA-DR expressas na superfície de monócitos/macrófagos diminuiu (medianas = 87,6; 84,0; 81,0; 85,0 e 80,0 respectivamente) em relação ao controle negativo (CN) (mediana=100,0) p=0,01. Todos os grupos tratados com EL aumentaram o número de linfócitos T auxiliares expressando moléculas CD28 (medianas = 90,9; 90,4; 91,5; 92,6 e 90,1 respectivamente) em relação ao CN (mediana=82,8) p=0,001 e também o número de moléculas CD152 expressas por células na superfície de linfócitos T auxiliares (medianas = 120,6; 108,8; 127,7; 114,6 e 121,3 respectivamente) em relação ao CN (mediana=100,0), p=0,03. Não foram encontradas diferenças estatísticas na expressão de moléculas CD80 e CD86 na superfície de monócitos/macrófagos cultivados com diferentes EL. Ainda não foram encontradas diferenças no número de linfócitos T auxiliares expressando CD152. Finalmente a expressão por células de moléculas CD28 na superfície de linfócitos T auxiliares também não mostrou alteração significante com as diferentes emulsões lipídicas. Conclusão: Emulsões lipídicas parenterais in vitro, diminuem a expressão de moléculas HLA-DR na superfície de monócitos/macrófagos e aumentam a expressão de moléculas CD28 e CD152 na superfície de linfócitos T auxiliares humanos. Estas alterações podem ser um dos mecanismos pelos quais as EL modulam funções de células imunes / HLA-DR and co-stimulatory molecules play a central role on leucocytes immune function. Different lipid emulsions (LE) may change leucocytes immune function. It is of interest to study the effect of different LE on HLA-DR and costimulatory molecules expression. To access the effect of LE on the HLA-DR, CD80 and CD86 expression on monocytes/macrophages (MO/MØ) surface and CD28 and CD152 (CD80/CD86 co-stimulatory molecules receptor) expression on human T helper lymphocytes (LØ CD4) surface we obtained mononuclear cells from peripheral blood of healthy volunteers (n=10) by using ficoll hypaque (d=1.077). The cells were cultured for 48 hours (MOMØ) and 72 hours (LØ CD4) and incubated with RPMI 1640 medium without (negative control) or added with 1mg/mL of commercial or experimental mixtures of five LE. Groups: a) NC - negative control without LE, b) LCTn-6 - n-6 polyunsaturated fatty acids (PUFA) rich LE ( soybean oil), c) LCTFO - 80% of LCT and 20% of n-3 PUFA rich LE (FO) (fish oil), d) MCT/LCT - LE containing 50% of medium chain triglycerides and 50% of n-6 PUFA rich LE, e) MCT/LCTFO - 80% of MCT/LCT LE and 20% of FO LE and f) SMOF - a new LE containing 30% of soybean oil, 30% of medium chain triglycerides, 25% of olive oil and 15% of fish oil. Mononuclear cells were activated by using 10?g/mL of phytohemagglutinin. Surface molecules expression was measured by flow cytometry. Percentage and intensity of fluorescence were recorded and the data were submitted to Friedman statistical test and Student-Newman-Keuls post test (p<0,05). Due the differences in basal expression between donors, prior to statistical tests, data from intensity of fluorescence were transformed of percentage relative of basal expression (where basal=100). All LE groups LCT, LCTFO, MCT/LCT, MCT/LCTFO and SMOF decreased HLA-DR intensity of fluorescence on monocytes/macrophages (mean= 87.6, 84.0, 81.0, 85.0, and 80.0 respectively) in relation to negative control (NC) (mean=100.0) cultured without LE (p=0,01). All LE groups increased the percentage of lymphocytes expressing CD28 (means=90.9, 90.4, 91.5, 92.6 and 90.1 respectively) in relation to control (mean=82.8) p=0,001 and CD152 intensity of fluorescence on lymphocytes cultured with all different LE (mean=120,6; 108,8; 127,7; 114,6 and 121,3 respectively) in relation to NC (mean=100,0), p=0,03. No significant differences were found on CD80 and CD86 expression on monocytes/macrophages surface, CD28 intensity of fluorescence and the percentage of lymphocytes expressing CD152 on lymphocytes cultured with the different studied LE. Conclusion: In vitro parenteral LE decreased HLA-DR expression on human monocytes/macrophages surface and increase co-stimulatory molecules receptor expression on human lymphocytes surface. These changes could be one of the mechanisms of LE modulation of immune cells functions

Ácidos graxos

Apresentação de antígeno

In vitro

Leucócitos mononucleares

Nutrição parenteral

Antigen presenting

Fatty acids

In vitro

Mononuclear leukocytes

Parenteral nutrition

Role of human gamma-delta T lymphocytes in the instruction of the adaptive immune response against Plasmodium falciparum infection. / Rôle des lymphocytes T gamma delta dans l’induction de la réponse immunitaire adaptative dans un contexte d’infection par Plasmodium falciparum.

Howard, Jennifer Ruth

16 July 2015

Les phosphoantigènes (P-Ag) de P. falciparum (P.f.) induisent une forte activation et une expansion des lymphocytes T (LT) Vγ9Vδ2 par un mécanisme encore mal décrit. Les LT Vγ9Vδ2 actives inhibent le cycle sanguin de P. f. par des médiateurs cytotoxiques solubles, inhibant ainsi la capacité invasive des mérozoites. Il a été montre in vitro que des LT Vγ9Vδ2 activés par les P-Ag peuvent présenter des antigènes et activer les LT αβ, agissant ainsi comme des cellules présentatrices d’antigènes (APC). Cette fonction n’a cependant pas été démontrée dans un contexte physiopathologique. Le but de ce projet est i) d’étudier les mécanismes d’activation des LT Vγ9Vδ2 par les stades sanguins P. f. et ii) d’evaluer le potentiel APC des LT Vγ9Vδ2 stimules par P. f. Nous montrons que l’activation des LT Vγ9Vδ2 par des globules rouges parasites par P. f. (GRP) intacts ne dépend ni d’un contact cellulaire, ni de l’expression de butyrophiline par le GRP. Les LT Vγ9Vδ2 sont activés par des molécules contenues dans les surnageants de culture de GRP, ayant les caractéristiques de P-Ags et étant libérées lors de la rupture des GRP. In vitro, les LT Vγ9Vδ2 stimules par les GRP expriment des marqueurs de surface associés à un rôle d’APC et cross-présentent un antigène modèle à une lignée T CD8 spécifique. In vivo, nous montrons une expression augmentée des marqueurs APC à la surface de LT Vγ9Vδ2 de patients infectés par P. falciparum. L’ensemble de ces données suggèrent que les P-Ag libérés par les GRP dans le milieu extracellulaire pourraient activer les LT Vγ9Vδ2 à distance, et ouvrent de nouvelles perspectives quant au rôle des LT Vγ9Vδ2 dans la réponse immunitaire adaptative anti-palustre. / P. falciparum derived phosphoantigens (P‐Ag) induce potent activation and expansion of Vγ9Vδ2 T-cells by a poorly described mechanism. Activated Vγ9Vδ2 T cells inhibit the Plasmodium falciparum blood cycle through soluble cytotoxic mediators, abrogating merozoite invasion capacity. In vitro, P-Ag activated Vγ9Vδ2 T lymphocytes have been shown to present antigens and induce αβ T lymphocyte responses, i.e. to act as an antigen presenting cell (APC). Whether this activity can be involved in a pathophysiological context is unknown. The aim of this PhD project is to a) investigate the mechanisms of Vγ9Vδ2 T cell activation by blood stage P. falciparum and b) assess the potential of P. falciparum activated Vγ9Vδ2 T cells to display APC functionality. We show that Vγ9Vδ2 T-cell activation by intact iRBCs is independent of iRBC contact and butyrophilin expression. Blood stage culture supernatants can potently activate Vγ9Vδ2 T-cells and bioactivity is found to be attributable to P-Ags released at the time of parasite egress from the RBC. In vitro iRBC stimulated Vγ9Vδ2 T cells up-regulate surface expression of APC associated markers and can cross-present a model antigen to specific CD8 T cell responders. In vivo we demonstrate an increase in surface expression of APC makers on Vγ9Vδ2 T cells from P. falciparum infected patients.Altogether, these data outline a framework whereby P‐Ag release by iRBC into extracellular milieu can promote activation of distant Vγ9Vδ2 T cells, and opens the door to a new aspect of Vγ9Vδ2 T cell contribution to P. falciparum adaptive immune responses.

Lymphocytes T Vγ9Vδ2

Plasmodium falciparum

Butyrophiline

Cellule présentatrice d’antigène

Vγ9Vδ2 T Lymphocytes

Plasmodium falciparum

Butyrophilin

Antigen presenting cells

Studium maternálně-fetálního mikrochimérismu APC s využitím MHCII/EGFP myšího modelu a clearovacích histologických technik / Study of the materno-fetal microchimerism of the APC using MHCII/EGFP mouse model and clearing histological techniques

Knížková, Karolina

January 2020

Microchimerism arises from the exchange of cells between genetically distinct individuals. The coexistence of genetically distinct cell populations within a single organism has possible effects on health and functioning of individuals immune systems, but the exact mechanisms of action are often not yet known. With the development of microscopic technologies and software for data analysis, the possibilities of detection and phenotyping of these rare cell populations are expanding. My intention in this work is to find maternal microchimerism in embryonic tissues (E13) and intestines of breastfed pups using MHCII/EGFP knock-in mouse model. Several different technologies potentially suitable for the detection of maternal microchimeric cells in offspring tissues (light sheet fluorescent microscopy - LSFM, virtual slide microscopy and flow cytometry) were selected. Advanced analysis of the obtained samples from the light sheet microscopy using the creation of a neural network was used here. The presence of maternal microchimerism was not demonstrated by flow cytometry. Using LSFM, image data were obtained from intestinal samples of suckling pups, which were processed by the neural network method. Data analysis of embryos (E13) obtained by the same method did not allow data analysis due to high...

Tolerance Induction to a Foreign Protein Antigen: Analysing the Role of B Cells in Establishing Peripheral Tolerance

Yuschenkoff, Victoria Nicole

14 September 1995

Tolerance to self proteins is largely dependent upon the deletion of immature, self-specific T and B cells in the thymus and bone marrow. Although highly efficient, the elimination of these self-reactive lymphocytes is dependent on the expression of their target antigen in these primary lymphoid organs. Many proteins, however, such as hormones, are developmentally regulated and expressed at different stages of life, while other proteins are expressed outside the thymus and marrow. To ensure self-tolerance, other mechanisms must exist to inactivate or prevent the activation of mature, potentially self-reactive lymphocytes and maintain peripheral tolerance. T cell activation requires direct recognition of a specific protein fragment, presented on the surface of an antigen presenting cell (APC), as well as the interaction between various T cell and APC surface molecules. In the absence of the costimulatory signals provided by these ligand-pair interactions and lymphokines, antigen recognition leads to T cell inactivation and tolerance to the protein. Since many autoimmune disorders appear to be based upon the aberrant activation of mature T lymphocytes, it is important to identify and understand the mechanisms of peripheral tolerance. The obvious importance of the APC in initiating the T cell immune response has led our lab to examine one of the many antigen-processing cells, the B lymphocyte. Our studies have shown that B cells are highly efficient APC and can present antigen at very low doses to cultured T cell lines. In addition, we have found that we can induce tolerance, as measured by a reduced antibody response to an immunogenic form of the protein, in naive, normal mice by targeting a foreign protein to their B cells for antigen processing and presentation. Tolerance in the treated mice can be traced to a lesion in the T cell compartment of the animals, thus suggesting that B cells can act as tolerizing APC for peripherally expressed antigens. To further explore this idea and find more direct evidence for the role of B cells in establishing peripheral tolerance, we developed a model system that would more closely resemble in vivo conditions. This thesis tests and provides additional evidence for the hypothesis that B cells are tolerizing antigen presenting cells for peripherally expressed protein antigens. Tolerance to the foreign protein human μ chain, is induced in normal recipient mice by the transfusion of splenocytes from transgenic mice that express the membrane-bound form of μ on their B cells. Tolerance is antigen-specific since the transfused recipients' antibody production to the irrelevant protein chicken IgG is not compromised. Only viable transgenic spleen cells are tolerogenic and even when human μ chain is accessible to other APCs for presentation, tolerance can be induced by the transfusion of live μ transgenic splenoctyes. These data suggested that the transfused μ chain-expressing B cells are the tolerizing APCs which was confirmed by experiments that compared the tolerizing abilities of purified B and T cells from the transgenic mice. Adoptive transfer experiments showed that the recipients' T cell response to human μ was impaired but an analysis of the isotypes produced by tolerized mice did not indicate that either helper T cell subset was specifically compromised. Splenocytes from human μ chain-secreting transgenic B cells also induce tolerance to human μ in nontransgenic mice. Although human μ chain-expressing B cells were not detected in transfused mice, the presence of measurable levels of human IgM in the sera of mice transfused with μ chain-secreting spleen cells suggests that the transfused transgenic B cells persist in their new host. In addition, the tolerizing ability of both resting and activated membrane-bound μ chain B cells was compared. Lipopolysaccharide (LPS)-activated transgenic spleen cells do not tolerize, nor do they prime for antibody to human μ, thus suggesting that the induction of costimulatory molecules on the transgenic B cells inhibits tolerance induction. To more specifically address this, human μ chain-expressing mice were bred to transgenic mice that express the costimulatory molecule, B7-1 (CD80), on their B cells. Double transgenic splenocytes, in which the B cells bear both human μ and B7-1, did not induce tolerance to human μ chain, a result that supports the idea that activated B cells are not tolerogenic. Together the data in this thesis show that resting B cells can process and present a foreign endogenous antigen in a tolerogenic manner to the immune system and suggest a role for the B cell in the maintenance of peripheral tolerance.

Antigen-Presenting Cells

B-Lymphocytes

T-Lymphocytes

Immunity, Cellular

Academic Dissertations

Dissertations, UMMS

Life Sciences

Medicine and Health Sciences

Primary Melanoma tumor immune contexture analysis: T regulatory cell to T effector cell ratio as related to MHC class II and GILT expression

Cole, Lauren

28 April 2017

A Thesis submitted to The University of Arizona College of Medicine - Phoenix in partial fulfillment of the requirements for the Degree of Doctor of Medicine. / Histopathologic examination of the tumor microenvironment demonstrates the presence of a vast repertoire of infiltrating lymphocytes and antigen presenting cells (APC’s). Recent studies establish a strong correlation between the tumor microenvironment cell composition and prognostic value in terms of cell type, location and ratio, referred to as a tumor’s immunoscore. More specifically, the relationship between T regulatory (Treg) cell to T effector (Teff) cell percentage predominates as a mechanism of tumor immune evasion. Further investigation of the factors influencing the development of Treg and Teff cells is therefore warranted. Gammainterferon‐inducible lysosomal thiol reductase (GILT) acts to influence antigenic processing and presentation by MHC class II cells, ultimately impacting lymphocyte development. Evaluation of the role of GILT expression in MHC class II+ APC’s with respect to Treg and Teff cell development in primary melanoma lesions, to our knowledge, has not been reported. Therefore our investigation focuses on elucidating a plausible relationship between GILT presence and Treg to Teff cell ratio. The aim of our study is to examine a possible association between GILT expression in APC’s and Treg:Teff cell ratio. We hypothesized GILT expression in melanoma cells would result in a decreased Treg to Teff ratio or an enhanced T cell‐mediated response. Our study included 17 de‐identified primary melanoma specimens previously stained and scored for Treg, Teff, CD8, MHC class II and GILT. Scoring was performed through identification of four areas per specimen with highest Treg and Teff cell density. These four areas were then averaged with ± standard deviation (SD). With use of landmark association, these four areas were identified and scored for MHC class II and GILT in APC’s and tumor cells with consideration to presence/absence, intensity and frequency of staining. Statistical significance was not reached relative to our hypothesized relationship of a decreased Treg to Teff cell ratio in the presence of GILT+ MHC class II. Similarly, we did not reach statistical significance when comparing individual cell types to GILT, MHC class II and GILT + MHC class. In our study, we were unable reach statistical significance relative to our proposed correlation between MHC class II and GILT presence leading to a decreased Treg to Teff cell ratio or enhanced T‐cell mediated immune response. A major limitation of our study included the small sample size leading to a probable type II error, prompting the need for further investigation of the factors influencing the Treg to Teff cell ratio within the melanoma tumor microenvironment on a larger scale.

Antigen-Presenting Cells

Tumor Microenvironment

T-effector Cells

T-Regulatory Cells

Immune Cell Contexture

MHC Class II cells

Melanoma

Role rodiny kináz Src v imunologických synapsích antigen prezentujících buněk. / The role of Src-family kinases in the immunological synapse of antigen presenting cells.

Kotlabová, Klára

January 2013

Antigen presentation during which antigen fragments in complex with MHC glycoproteins are recognized by T cell antigen-specific receptors is necessary for the initiation of adaptive immune response. During this process, immunological synapse is assembled at the site of contact between the T cell and the antigen-presenting cell (APC). This leads to the activation of receptors on the surface of both cells followed by triggering of multiple signaling pathways. However, our knowledge about the signaling occurring at the APC-side of the IS is limited in comparison to the T cell side. Here, we analyze role of Src family kinases in the APC signaling pathways. For this purpose, constructs targeting Csk kinase to the plasma membrane of APCs were prepared to inhibit SFKs there. We show that expression of these constructs inhibits activation of SFKs, calcium mobilization and cell activation of K46 B cell line. Further, expression of these constructs in hematopoietic progenitors attenuates their differentiation into dendritic cells which then results in their decreased ability to stimulate T cells.

Caracterização da resposta imune in situ nas lesões de hanseníase indeterminada / Characterization of the in situ immune response in indeterminate leprosy lesions

Alvarenga, Marcia Lanzoni de

17 August 2015

A forma indeterminada é a fase inicial da hanseníase, que se caracteriza histologicamente pelo infiltrado inflamatório leve, não granulomatoso, de linfócitos e histiócitos ao redor de vasos, anexos e nervos. No local de entrada do M. leprae, as células apresentadoras de antígeno do tipo células dendríticas são as primeiras a encontrar o bacilo. Este, no interior de células dendríticas, desencadeia a produção local de citocinas e quimiocinas, que resultam em proliferação de linfócitos T helper 1 ou T helper 2, assim definindo uma resposta imune celular ou humoral, respectivamente. As lesões tuberculoides mostram predominância das citocinas de padrão Th1 como IL-2, TNF-alfa, IFN-y, IL-12 e IL-18, enquanto que nas lesões virchowianas predominam citocinas de padrão Th2, como IL-4, IL-5, IL-10 e TGF-beta. Na pele, as principais células dendríticas são células dendríticas mieloides, células de Langerhans e alguns dendrócitos dérmicos. São identificadas respectivamente pela expressão imuno-histoquímica de S100, CD1a e Fator XIIIa. Células de Langerhans e dendrócitos dérmicos Fator XIIIa positivos estão aumentados em quantidade nas lesões tuberculoides quando comparadas com lesões virchowianas. Os objetivos do presente estudo foram: 1) caracterizar a inflamação \"in situ\" na hanseníase indeterminada através da quantificação das marcações imuno-histoquímicas de: CD57, CD4, CD8, CD1a, S100, FXIIIa, CD68, Foxp3, CD123, IL-1, IL-2r, IL-4, IL-6, IL-8, IL-10, IL-12, IL-18, IFN-, TNF-alfa, TGF-beta, iNOS, granzima B, receptor Toll-like 2/4, e antígeno BCG, 2) comparar o perfil fenotípico e citocínico das lesões na hanseníase indeterminada entre grupos de reação de Mitsuda positiva e negativa, a fim de investigar se existem padrões que possam prever para qual forma a doença evoluiria, e 3) revisar a histopatologia da forma indeterminada através da análise semiquantitativa das alterações vistas à coloração de hematoxilina/eosina. Foram selecionadas 15 lesões de pacientes com hanseníase indeterminada. Foram usados grupos controles de expressão de Fator XIIIa e CD1a em 10 casos de pele normal. A histopatologia mostrou discretas alterações epidérmicas, como alteração vacuolar e exocitose de linfócitos (33% dos casos cada), apoptose de queratinócitos (26%), atrofia e acantose (06% dos casos cada); infiltrado inflamatório linfomononuclear neural (100%), perivascular superficial (100%), perivascular profundo (93%), peri-écrino (40%) e peri-folículo pilossebáceo (20%), além de melanófagos em 93% dos casos. Esses achados mostraram que nem sempre todos os ambientes estão acometidos por inflamação na histopatologia. Em 66% dos pacientes foi encontrado antígeno bacilar (por Fite-Faraco ou técnica imuno-histoquímica anti-BCG), portanto a forma indeterminada não deve ser considerada sistematicamente como paucibacilar. Não houve diferença significativa de padrões de marcadores entre os grupos Mitsuda positivo e negativo. No microambiente inflamatório das lesões houve expressões significativas de TLR 2/4, Fator XIIIa, CD4, CD8, IL-2r, IL-4, IL-10, iNOS e TGF-beta. A expressão importante de IL-4, IL-10 e TGF- beta nas lesões de hanseníase indeterminada significaram tendência de resposta imune para o polo Th2, um ambiente de tolerância à permanência do bacilo. A baixa expressão de IFN-y colaborou para a inexpresiva resposta Th1. Não houve diferença significativa na expressão de CD1a entre as lesões e pele normal. Fator XIIIa foi expresso em mais que 50 células/mm2 em todos os casos, com quantidades significativamente maiores que outras células dendríticas nas lesões (S100, CD68, CD123) e que a pele normal. Estes achados demonstraram a importância dos dendrócitos dérmicos Fator XIIIa positivos na apresentação de antígeno na fase inicial da hanseníase / The indeterminate form is the initial stage of leprosy, which is characterized histologically by mild inflammatory infiltrate, non granulomatous, with lymphocytes and histiocytes around vessels, nerves and adnexals. When M. leprae enter the host, antigen-presenting cells of dendritic type are the first cells to find the bacillus. Once inside dendritic cells, the bacillus elicits local production of cytokines and chemokines, which result in proliferation of T lymphocytes helper 1 or T helper 2, thereby defining a cellular or humoral immune response, respectively. The tuberculoid lesions show predominance of Th1 cytokines such as IL-2, TNF-alfa, IFN-y, IL-12 and IL-18, whereas in the lepromatous lesions predominate cytokines of Th2 pattern such as IL-4, IL-5 IL-10 and TGF-beta. In the skin, main dendritic cells are myeloid dendritic cells, Langerhans cells, and some dermal dendrocytes. They are identified respectively by immunohistochemical expression of S100, CD1a and Factor XIIIa. Langerhans cells and dermal dendrocytes Factor XIIIa positive are increased in number in tuberculoid lesions compared with lepromatous lesions. The objectives of this study were: 1) to characterize \"in situ\" inflammation in indeterminate leprosy through the quantification of immunohistochemical markers: CD57, CD4, CD8, CD1a, S100, FXIIIa, CD68, Foxp3, CD123, IL-1, IL-2r, IL-4, IL-6, IL-8, IL-10, IL-12, IL-18, IFN-y, TNF-alfa, TGF-beta, iNOS, granzyme B, Toll-like receptor 2/4, and BCG antigen, 2) compare the phenotypic and cytokinic profile of indeterminate leprosy lesions between positive and negative Mitsuda reaction groups in order to investigate if there are patterns that can predict which way the disease may evolve, and 3 ) review the histopathology of the indetermate form by semi-quantitative analysis of changes seen in hematoxylin / eosin. Fifteen lesions of patients with indeterminate leprosy were selected. There was used control groups of Factor XIIIa and CD1a expression in 10 cases of normal skin. Histopathology showed discrete epidermal changes, such as vacuolar changes and lymphocyte exocytosis (in 33% of cases each), keratinocyte apoptosis (26%), atrophy and acanthosis (in 06% of cases each); neural lymphocytic inflammatory infiltrate (100%), superficial perivascular (100%), deep perivascular (93%), peri-eccrine (40%), peri-pilosebaceous follicle (20%), and melanophages in 93% of cases. These findings showed that not always all environments are affected by inflammation in histopathology. In 66% of patients it was found bacterial antigen (by Fite-Faraco or immunohistochemical technique anti-BCG), so the indeterminate form should not be systematically considered as paucibacillary. There was no significant difference in phenotypic and cytokinic patterns between the positive and negative Mitsuda groups. In the microenvironment of inflammatory lesions there was significant expression of TLR 2/4, Factor XIIIa, CD4, CD8, IL-2r, IL-4, IL-10, TGF-beta and iNOS. The important expression of IL-4, IL-10 and TGF-beta in indeterminate leprosy meant tendency to Th2 immune response pole, an environment of tolerance to permanence of bacillus. Low IFN-? expression contributed to the negligible Th1 response. There was no significant difference in the expression of CD1a between the lesions and normal skin. Factor XIIIa was expressed as greater than 50 cells / mm2 in all cases, with significantly larger quantities than other dendritic cells in lesions (S100, CD68, CD123) and than normal skin. These findings demonstrate the importance of Factor XIIIa positive dermal dendrocytes in antigen presentation at the initial stage of leprosy

Antigen-presenting cells

Células apresentadoras de antígenos

Células dendríticas

Células Th2

Dendritic cells

Factor XIIIa

Fator XIIIa

Hanseníase paucibacilar

Leprosy paucibacillary

Th2 cells

Caracterização da resposta imune in situ nas lesões de hanseníase indeterminada / Characterization of the in situ immune response in indeterminate leprosy lesions

Marcia Lanzoni de Alvarenga

17 August 2015

A forma indeterminada é a fase inicial da hanseníase, que se caracteriza histologicamente pelo infiltrado inflamatório leve, não granulomatoso, de linfócitos e histiócitos ao redor de vasos, anexos e nervos. No local de entrada do M. leprae, as células apresentadoras de antígeno do tipo células dendríticas são as primeiras a encontrar o bacilo. Este, no interior de células dendríticas, desencadeia a produção local de citocinas e quimiocinas, que resultam em proliferação de linfócitos T helper 1 ou T helper 2, assim definindo uma resposta imune celular ou humoral, respectivamente. As lesões tuberculoides mostram predominância das citocinas de padrão Th1 como IL-2, TNF-alfa, IFN-y, IL-12 e IL-18, enquanto que nas lesões virchowianas predominam citocinas de padrão Th2, como IL-4, IL-5, IL-10 e TGF-beta. Na pele, as principais células dendríticas são células dendríticas mieloides, células de Langerhans e alguns dendrócitos dérmicos. São identificadas respectivamente pela expressão imuno-histoquímica de S100, CD1a e Fator XIIIa. Células de Langerhans e dendrócitos dérmicos Fator XIIIa positivos estão aumentados em quantidade nas lesões tuberculoides quando comparadas com lesões virchowianas. Os objetivos do presente estudo foram: 1) caracterizar a inflamação \"in situ\" na hanseníase indeterminada através da quantificação das marcações imuno-histoquímicas de: CD57, CD4, CD8, CD1a, S100, FXIIIa, CD68, Foxp3, CD123, IL-1, IL-2r, IL-4, IL-6, IL-8, IL-10, IL-12, IL-18, IFN-, TNF-alfa, TGF-beta, iNOS, granzima B, receptor Toll-like 2/4, e antígeno BCG, 2) comparar o perfil fenotípico e citocínico das lesões na hanseníase indeterminada entre grupos de reação de Mitsuda positiva e negativa, a fim de investigar se existem padrões que possam prever para qual forma a doença evoluiria, e 3) revisar a histopatologia da forma indeterminada através da análise semiquantitativa das alterações vistas à coloração de hematoxilina/eosina. Foram selecionadas 15 lesões de pacientes com hanseníase indeterminada. Foram usados grupos controles de expressão de Fator XIIIa e CD1a em 10 casos de pele normal. A histopatologia mostrou discretas alterações epidérmicas, como alteração vacuolar e exocitose de linfócitos (33% dos casos cada), apoptose de queratinócitos (26%), atrofia e acantose (06% dos casos cada); infiltrado inflamatório linfomononuclear neural (100%), perivascular superficial (100%), perivascular profundo (93%), peri-écrino (40%) e peri-folículo pilossebáceo (20%), além de melanófagos em 93% dos casos. Esses achados mostraram que nem sempre todos os ambientes estão acometidos por inflamação na histopatologia. Em 66% dos pacientes foi encontrado antígeno bacilar (por Fite-Faraco ou técnica imuno-histoquímica anti-BCG), portanto a forma indeterminada não deve ser considerada sistematicamente como paucibacilar. Não houve diferença significativa de padrões de marcadores entre os grupos Mitsuda positivo e negativo. No microambiente inflamatório das lesões houve expressões significativas de TLR 2/4, Fator XIIIa, CD4, CD8, IL-2r, IL-4, IL-10, iNOS e TGF-beta. A expressão importante de IL-4, IL-10 e TGF- beta nas lesões de hanseníase indeterminada significaram tendência de resposta imune para o polo Th2, um ambiente de tolerância à permanência do bacilo. A baixa expressão de IFN-y colaborou para a inexpresiva resposta Th1. Não houve diferença significativa na expressão de CD1a entre as lesões e pele normal. Fator XIIIa foi expresso em mais que 50 células/mm2 em todos os casos, com quantidades significativamente maiores que outras células dendríticas nas lesões (S100, CD68, CD123) e que a pele normal. Estes achados demonstraram a importância dos dendrócitos dérmicos Fator XIIIa positivos na apresentação de antígeno na fase inicial da hanseníase / The indeterminate form is the initial stage of leprosy, which is characterized histologically by mild inflammatory infiltrate, non granulomatous, with lymphocytes and histiocytes around vessels, nerves and adnexals. When M. leprae enter the host, antigen-presenting cells of dendritic type are the first cells to find the bacillus. Once inside dendritic cells, the bacillus elicits local production of cytokines and chemokines, which result in proliferation of T lymphocytes helper 1 or T helper 2, thereby defining a cellular or humoral immune response, respectively. The tuberculoid lesions show predominance of Th1 cytokines such as IL-2, TNF-alfa, IFN-y, IL-12 and IL-18, whereas in the lepromatous lesions predominate cytokines of Th2 pattern such as IL-4, IL-5 IL-10 and TGF-beta. In the skin, main dendritic cells are myeloid dendritic cells, Langerhans cells, and some dermal dendrocytes. They are identified respectively by immunohistochemical expression of S100, CD1a and Factor XIIIa. Langerhans cells and dermal dendrocytes Factor XIIIa positive are increased in number in tuberculoid lesions compared with lepromatous lesions. The objectives of this study were: 1) to characterize \"in situ\" inflammation in indeterminate leprosy through the quantification of immunohistochemical markers: CD57, CD4, CD8, CD1a, S100, FXIIIa, CD68, Foxp3, CD123, IL-1, IL-2r, IL-4, IL-6, IL-8, IL-10, IL-12, IL-18, IFN-y, TNF-alfa, TGF-beta, iNOS, granzyme B, Toll-like receptor 2/4, and BCG antigen, 2) compare the phenotypic and cytokinic profile of indeterminate leprosy lesions between positive and negative Mitsuda reaction groups in order to investigate if there are patterns that can predict which way the disease may evolve, and 3 ) review the histopathology of the indetermate form by semi-quantitative analysis of changes seen in hematoxylin / eosin. Fifteen lesions of patients with indeterminate leprosy were selected. There was used control groups of Factor XIIIa and CD1a expression in 10 cases of normal skin. Histopathology showed discrete epidermal changes, such as vacuolar changes and lymphocyte exocytosis (in 33% of cases each), keratinocyte apoptosis (26%), atrophy and acanthosis (in 06% of cases each); neural lymphocytic inflammatory infiltrate (100%), superficial perivascular (100%), deep perivascular (93%), peri-eccrine (40%), peri-pilosebaceous follicle (20%), and melanophages in 93% of cases. These findings showed that not always all environments are affected by inflammation in histopathology. In 66% of patients it was found bacterial antigen (by Fite-Faraco or immunohistochemical technique anti-BCG), so the indeterminate form should not be systematically considered as paucibacillary. There was no significant difference in phenotypic and cytokinic patterns between the positive and negative Mitsuda groups. In the microenvironment of inflammatory lesions there was significant expression of TLR 2/4, Factor XIIIa, CD4, CD8, IL-2r, IL-4, IL-10, TGF-beta and iNOS. The important expression of IL-4, IL-10 and TGF-beta in indeterminate leprosy meant tendency to Th2 immune response pole, an environment of tolerance to permanence of bacillus. Low IFN-? expression contributed to the negligible Th1 response. There was no significant difference in the expression of CD1a between the lesions and normal skin. Factor XIIIa was expressed as greater than 50 cells / mm2 in all cases, with significantly larger quantities than other dendritic cells in lesions (S100, CD68, CD123) and than normal skin. These findings demonstrate the importance of Factor XIIIa positive dermal dendrocytes in antigen presentation at the initial stage of leprosy

Células apresentadoras de antígenos

Células dendríticas

Células Th2

Fator XIIIa

Hanseníase paucibacilar

Antigen-presenting cells

Dendritic cells

Factor XIIIa

Leprosy paucibacillary

Th2 cells

Identification of the peripheral niche controlling CD4 homeostatic proliferation.

Zaid, Intesar

06 1900

No description available.

CD4.

Cellules dendritiques

Interleukine-7

Cellules présentatrices d'antigènes

Dendritic cells

Interleukin-7

Antigen presenting cells

Lymphocytes

UVA/Riboflavin-Induced Apoptosis in Mouse Cornea

Wang, Fan

13 February 2014

Background: A mouse model of combined UVA/riboflavin irradiation to eliminate stromal cells and other antigen-presenting cells in the cornea provides the basis for a probably low risk of corneal transplantation. Methods: After abrasion of the epithelium, the central corneas of mouse eyes were treated with UVA/riboflavin in vitro. Histological studies of hematoxylin-eosin and immunohistochemical staining with caspase 3 were performed. Dissected mouse corneas were analyzed by Western blot. Results: Apoptotic cells were shown on the central corneal stroma; a cell-free zone was displayed in the cornea. Numbers of dead cells increased according to cultivation time. However, the endothelium survived due to the adjustment of the irradiation dose. Conclusions: A cell-free zone in the stroma of the mouse cornea was produced by UVA/riboflavin irradiation in vitro. The technique makes possible to prevent or reduce immunological reactions and the risk of graft rejection by pretreatment of the donor cornea, ultimately prolonging graft survival. / Dieser Beitrag ist mit Zustimmung des Rechteinhabers aufgrund einer (DFG-geförderten) Allianz- bzw. Nationallizenz frei zugänglich.

UV-Bestrahlung

Riboflavin

Vorbehandlung

antigenpräsentierende Zellen

Kornea

Hornhaut

Apoptose

Ultraviolet irradiation

Riboflavin pretreatment

Antigen-presenting cells

Cornea

Apoptosis

ddc:610

rvk:XA 10000