Cannabinoids induce immunoglobulin class switching to IgE in B lymphocytes

Agudelo, Marisela.

January 2009

Dissertation (Ph.D.)--University of South Florida, 2009. / Title from PDF of title page. Document formatted into pages; contains 92 pages. Includes vita. Includes bibliographical references.

B-cell-survival factors in multiple sclerosis and myasthenia gravis /

Thangarajh, Mathula,

January 2007

Diss. (sammanfattning) Stockholm : Karolinska institutet, 2007. / Härtill 5 uppsatser.

Regulation of transcription and analysis of drug targets in lymphoma and myeloma cells /

Bolick, Sophia C. E.

January 2006

Dissertation (Ph.D.)--University of South Florida, 2006. / Includes vita. Includes bibliographical references (leaves 119-141). Also available online.

Analysis of the role of FCRL5 and FIGLERs in B cell development, signaling and malignancy

Haga, Christopher L.

January 2008

Thesis (Ph. D.)--University of Alabama at Birmingham, 2008. / Title from first page of PDF file (viewed June 6, 2008). Includes bibliographical references.

B cell signaling and bioinformatics : revealing components of the MHC class II antigen processing and presentation pathway

Lee, Jamie Ann.

January 2005

Thesis (Ph. D.) -- University of Texas Southwestern Medical Center at Dallas, 2005. / Vita. Bibliography: 195-256.

Analysis of Low Zone Tolerance in Normal and B Cell-Deficient Mice

Baird, Allison Michelle

26 April 1996

This thesis investigates the role of B cells as antigen-specific antigen-presenting cells (APC) in self tolerance to low concentrations of soluble self proteins and in acquired tolerance to low doses of soluble foreign protein antigens. Experiments were performed in normal and B cell-deficient animals, and tolerance induction was measured by T cell proliferation assays. T cell proliferation was reduced in B cell-deficient mice, indicating that B cells may be involved in efficient activation of naive T cells in response to protein antigen both in vivo and in vitro. To study acquired tolerance induced by low doses of soluble foreign protein antigen, normal and B cell-deficient adult mice were injected intravenously with repeated low doses (10 μg) of deaggregated ovalbumin (OVA), and then challenged with OVA in complete Freund's adjuvant. In animals treated with deaggregated OVA, the in vitro proliferative responses of LN T cells to OVA were significantly reduced, and production of the Th1 cytokine, IFN-γ, in response to OVA was lost. This occurred in both normal and B cell-deficient treated animals, indicating that B cell antigen presentation was not required for this phenomenon. B cells were also unnecessary for self tolerance of T cells to the transgenic self antigen, hen egg lysozyme (HEL), in a transgenic mouse strain with very low serum lysozyme concentration. Partial low zone tolerance induced by deaggregated, low-dose OVA was selective for the Th1 response, as measured by in vitro proliferation and IL-2 and IFN-γ production, because antibody responses of normal mice to this T cell-dependent antigen were largely unaffected. Both treated and untreated animals produced equivalent titers of anti-OVA antibodies, predominantly of the IgG1 and IgG2b isotypes, following challenge with OVA in complete Freund's adjuvant. Tolerance to low levels of the transgenic HEL self protein in mice expressing different MHC molecules was also addressed. Transgenic mice that were H-2b/b in the class II region were not tolerant to the transgenic self protein, whereas transgenic mice of the H-2b/k were tolerant.

Antigen-Presenting Cells

B-Lymphocytes

Immunity

Cellular

Mice

Amino Acids, Peptides, and Proteins

Animal Experimentation and Research

Biological Factors

Cells

Hemic and Immune Systems

Modulação da reação de hipersensibilidade tipo I por células apresentadoras de antígenos de camundongos tratados com Propionibacterium acnes ou seu polissacarídeo solúvel / Modulation of type I hypersensitivity reaction by antigen presenting cells from mice treated with Propionibacterium acnes or its soluble polysaccharide

Squaiella-Baptistão, Carla Cristina [UNIFESP]

25 March 2009

Made available in DSpace on 2015-07-22T20:50:27Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-03-25 / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / Dentre os efeitos moduladores da Propionibacterium acnes (P. acnes), um de grande importância, verificado em nosso laboratório em um modelo murino de hipersensibilidade imediata à ovoalbumina (OVA), é a sua capacidade de direcionar a resposta imune para Th1 ou Th2, dependendo do esquema de tratamento dos animais. Efeito semelhante foi induzido pelo polissacarídeo solúvel extraído da bactéria (PS), porém, como apenas a sua capacidade de modular a resposta Th1 havia sido verificada, nós nos propusemos a investigar, no presente estudo, se o PS poderia também potencializar a resposta Th2. De fato, verificamos que o polissacarídeo solúvel extraído da P. acnes foi capaz de potencializar a reação de hipersensibilidade imediata na pata de camundongos, como demonstrado pelo aumento do número de eosinófilos no infiltrado inflamatório, predominância do número de esplenócitos produtores de IL-4 e aumento da produção de IgG1 anti-OVA, concomitantemente à diminuição de IgG2a, compatível com padrão Th2 de resposta. Além disso, nós também avaliamos se os efeitos de potencialização ou supressão da hipersensibilidade imediata induzidos pela P. acnes ou seu polissacarídeo estariam relacionados com diferenças no número e grau de ativação de células apresentadoras de antígenos (APCs) e linfócitos B1. Observamos que o aumento da quantidade de APCs esplênicas positivas para moléculas co-estimuladoras, TLR4 e IL-4 em animais tratados com P. acnes ou PS e a maior expressão de CD80 por linfócitos B1c peritoneais estava relacionada com exacerbação da resposta Th2. Por outro lado, o aumento do número de linfócitos B2 esplênicos TLR2+, bem como maior expressão de TLR9 intracelular por células dendríticas, e também menor número de células B1a peritoneais positivas para TLR2 e TLR9 intracelular em camundongos tratados com P. acnes ou PS, estava relacionado com supressão da reação. Quanto à síntese de citocinas, verificou-se um aumento menos pronunciado do número de APCs IL-4+ e também maior quantidade de células produtoras de IL-12 nos grupos em que a reação foi suprimida, em relação aos submetidos ao protocolo de exacerbação. In vitro, o estímulo concomitante de P. acnes e OVA em co-culturas de células dendríticas e linfócitos T aumentou a liberação de IL-5 e IL-17, em relação às culturas estimuladas apenas com OVA, e o estímulo concomitante de PS e OVA aumentou a síntese de IL-17. Já o estímulo com P. acnes ou PS, seguido do estímulo com OVA no dia seguinte, induziu uma diminuição da liberação de IL-5 e IL-17, em comparação com as culturas estimuladas apenas com OVA, sugerindo que a P. acnes e o polissacarídeo atuam diretamente sobre células apresentadoras de antígenos. / Among Propionibacterium acnes (P. acnes) immunomodulatory effects, one of great importance, verified in our laboratory in a murine model of type I hypersensitivity to ovalbumin (OVA), is its capacity to direct the immune response to Th1 or Th2, depending on the animals treatment. Similar effect was induced by the soluble polysaccharide extracted from the bacteria (PS), however, since only its capacity to modulate the Th1 response has been verified, we decided to investigate, in the present study, if PS could also potentiate the Th2 response. In fact, this compound was able to potentiate or suppress the immediate hypersensitivity reaction in mice, depending on the protocol used. Besides, we investigated, in this work, whether the number of spleen cells and peritoneal B1 lymphocytes would be different between the treatment protocols, being related to potentiation or suppression of the OVA response, and also if the activation status of antigen presenting cells (APCs) and B1 lymphocytes could interfere on reaction modulation. We verified that the higher numbers of APCs expressing co-stimulatory molecules and the higher expression levels of these molecules on cell surface are probably related to potentiation of the Th2 response to OVA induced by P. acnes or PS. The higher CD80 expression by peritoneal B1c lymphocytes is also possibly involved with OVA response exacerbation in these animals. Besides, there seems to be a correlation between higher number of APCs expressing TLR4 and exacerbation of the immediate hypersensitivity reaction in P. acnes- or PS-treated mice. Differences on TLRs expression by spleen and peritoneal B1 lymphocytes can also be related to the type I hypersensitivity modulation. Analysis of cytokines synthesis by spleen APCs confirmed the Th2 potentiation or suppression in this model. Finally, in vitro experiments using co-cultures of dendritic cells and T lymphocytes indicated that P. acnes and PS seem to perform their effects of Th2 response potentiation or suppression by direct action on antigen presenting cells. / TEDE / BV UNIFESP: Teses e dissertações

Propionibacterium acnes

Células apresentadoras de antígenos

Linfócitos B

Hipersensibilidade tipo I

Imunomodulação

Hipersensibilidade imediata

Propionibacterium acnes

Antigen-presenting cells

B-Lymphocytes

Hypersensitivity, immediate

Immunomodulation

Virus-Lymphocyte Interactions: Virus Expression Is Differentially Modulated by B Cell Activation Signals: A Dissertation

Schmidt, Madelyn R.

01 January 1991

It is shown here that the ability of B lymphocytes to act as supportive host cells for virus infections requires they be activated from the resting Gostage of the cell cycle. I have used a series of activation regimens, which allow B cells to progress to different stages in their activation/differentiation pathway toward antibody secretion, in order to evaluate the extent of activation required to support vesicular stomatitis or Newcastle disease virus infections. At least three distinct phases during B cell activation which affected VSV infection were defined. Freshly isolated resting murine splenic B cells in the Go phase of the cell cycle do not support VSV, assessed by protein synthesis, infectious center formation, and PFU production. Small B cells cultured for 48 hours without stimulation still do not support VSV. B cells stimulated with the lymphokines found in Con A activated supernatants from splenic T cells or cloned T cell lines transited into the G1 phase of the cell cycle but remain refractory to VSV. These VSV non-supportive B cell populations do take up virus particles and transcribe viral mRNAs which can be translated in vitro, suggesting a translational block to VSV. B cells stimulated into the S phase of the cell cycle with anti-immunoglobulin synthesize VSV proteins and increased numbers of infectious centers, but only low level PFU synthesis (center) is observed. Co-stimulation with anti-Ig and lymphokines, which supports differentiation to antibody secretion, enhanced PFU synthesis without further increasing the number of infected B cells. LPS, which activates B cells directly to antibody secretion by a pathway different from anti-Ig, induced infectious centers, and PFUs at levels comparable to those seen when stably transformed permissive cell lines are infected. Co-stimulation of LPS activated B cells with the same lymphokine populations that enhance PFU production when anti-Ig is used as a stimulator suppresses PFU production completely, suggesting that anti-Ig and LPS activated B cells are differentially responsive to lymphokines. NDV infection of murine B cells differed markedly from VSV infection, as all B cell populations examined gave a similar response pattern. NDV viral proteins were synthesized by B cells in each of the activation states previously described, even freshly isolated B cells. Infectious center formation increased up to 5-fold over the levels observed with unstimulated B cells after anti-Ig or LPS activation. However, PFU synthesis was low (center) for all B cell populations. These results suggest that these two similar viruses may be dependent on different host cell factors and that these factors are induced for VSV but not NDV by the B cell activators employed here or that the process of infection of B cell by these two viruses induces different cellular responses.

Cell Communication

B-Lymphocytes

Viruses

Newcastle Disease Virus

Amino Acids, Peptides, and Proteins

Animal Diseases

Cells

Hemic and Immune Systems

Stomatognathic Diseases

Virus Diseases

Estudo molecular da via extrínseca da apoptose em indivíduos com imunodeficiência comum variável. / Molecular study of extrinsec apoptosis pathway in patients with Common Variable Immunodeficiency.

Lilian Cristina Buzzetto

24 May 2012

A Imunodeficiência de Variável Comum (ICV) é caracterizada por baixos níveis de imunoglobulinas com susceptibilidade a. Analisamos a distribuição de linfócitos, apoptose espontânea e a expressão gênica de receptores de morte, ligantes, adaptadores, moléculas reguladoras, inibidoras e anti-apotóticas em células CD4+ e CD8+ de 19 pacientes ICV e 19 controles. Pacientes com ICV apresentam diminuição na frequência de linfócitos TCD4+ e CD4+CD45RA+ e menor relação CD4/CD8 que indivíduos saudáveis. O grupo de pacientes mostrou maior frequência de apoptose espontânea em linfócitos totais e CD4+. Células CD4+ dos indivíduos afetados apresentaram menor expressão gênica de TRAIL-R, BCL-2, FLIPL e FADD; células CD8+ apresentaram diminuição da expressão gênica de TRAIL, FADD, BCL-2, BCL -xL e um aumento de FLIPs. Os resultados sugerem um desequilíbrio nos mecanismos que controlam a apoptose de linfócitos nestes pacientes, o que pode ajudar a elucidar as alterações observadas no compartimento de células T dos pacientes com ICV. / Common Variable Immunodeficiency (CVID) is is characterized by low immunoglobulins levels with susceptibility to infections. We have analyzed T cell distribution and spontaneous apoptosis in peripheral blood of CVID, as well as gene expression of several molecules involved in apoptosis, including death receptors, ligands, adapters, regulatory and anti-apototic molecules in CD4+ and CD8+ cells of 19 CVID patients and 19 healthy subjects. CVID subjects present decreased frequency of TCD4+ and CD4+ CD45RA+ cells and lower CD4/CD8 ratio than healthy controls. CVID group also presented higher frequency of spontaneous apoptosis in lymphocytes and CD4+ cells. CD4+ showed lower expression of TRAIL-R, BCL-2, FLIPL and FADD; CD8+ cells presented lower expression of TRAIL, FADD, BCL-2, BCL-xL and a augment of FLIP. Results suggest an imbalance in mechanisms controlling cell death of those patients lymphocytes, which might help to elucidate the changes observed in T cell compartment of CVID patients.

Apoptose

Células mononucleares

imunodeficiência comum variável

imunofenotipagem

imunologia celular

imunologia clínica

linfócitos B

Apoptosis

B lymphocytes

Cellular immunology

Clinical Immunology

Common variable immunodeficiency

Immunophenotyping

Mononuclear cells

Análise da detecção de C4d, linfócitos B e plasmócitos no processo de rejeição ao aloenxerto renal / Analysis of C4d, B lymphocytes and plasma cells detection in the renal allograft rejection

Hugo Ludovico Martins

07 April 2010

A rejeição ao aloenxerto mediada por mecanismos celulares ou humorais representa uma importante complicação no pós-transplante renal. Estudos anteriores demonstraram que o depósito de C4d peritubular é um marcador de rejeição mediada por anticorpos. A técnica padrão ouro para a pesquisa de C4d é a imunofluorescência em criostato. No entanto, o manuseio do material congelado implica em algumas limitações custo-operacionais, particularmente em nosso meio. Nos casos de rejeição mediada por anticorpos é de relevância patogenética a análise da participação de linfócitos B e plasmócitos, pois são as células responsáveis pela produção de anticorpos. Considerando que até o momento o envolvimento de linfócitos B e plasmócitos no processo de rejeição foi pouco investigado, no presente estudo também será analisada a expressão de CD20 e CD138 em biópsias renais, para caracterização destes componentes celulares. Portanto, o objetivo do presente estudo foi analisar a detecção do fragmento C4d por meio de 4 diferentes técnicas, além de analisar o infiltrado de linfócitos B e plasmócitos em biópsias de enxerto renal, correlacionando estes achados com o C4d peritubular. Foram analisadas 107 biópsias de 82 pacientes submetidos a transplante renal. A pesquisa do C4d foi realizada utilizando-se as técnicas de imunofluorescência [IF] (em cortes de criostato e de parafina) e imuno-histoquímica [IH] (em cortes de criostato e de parafina), enquanto que as pesquisas dos linfócitos B e plasmócitos foram realizadas pela técnica de IH em cortes de parafina utilizando-se os anticorpos anti-CD20 e anti-CD138, específicos para linfócitos B e plasmócitos, respectivamente. Com relação à detecção de C4d, as técnicas com maior índice de concordância com a IF-criostato, considerada padrão-ouro, foram IH-criostato (75,6% dos casos apresentaram resultados coincidentes, r=0,72; p<0,0001) e IF-parafina (73%, r=0,59; p=0,0001), enquanto a taxa de concordância na técnica de IH-parafina foi de apenas 51,4% (r=0,35; p=0,03). Analisando a evolução clínica, a sobrevida do enxerto renal em 3 anos pós-biópsia foi menor no grupo C4d positivo comparado ao grupo C4d negativo (67% vs 96%, respectivamente, p=0,01). A prevalência de linfócitos B (CD20+) foi de 54% das biópsias de enxerto renal. A análise histológica do infiltrado de linfócitos B revelou 2 padrões distintos de infiltrado: padrão de células isoladas (74%) e padrão nodular (26%). O padrão nodular esteve associado a uma menor sobrevida do enxerto renal em 3 anos pós-biópsia (61% vs 89% no grupo CD20 negativo; p=0,03; e 61% vs 87% no grupo padrão de células isoladas; p=0,03). A prevalência de plasmócitos (CD138+) em biópsias de enxerto renal foi de 59%. O infiltrado plasmocitário não esteve associado a uma pior evolução clínica do transplante. A análise da correlação entre C4d peritubular, linfócitos B e plasmócitos demonstrou que o número de células CD20+ e CD138+ foi significativamente maior nos casos C4d positivos comparados aos casos C4d negativos (CD20+: 155±53 vs 26±7 cels/mm2, respectivamente; p=0,001; CD138+: 46±22 vs 4±1 cels/mm2, respectivamente; p=0,002). O presente estudo concluiu que o depósito peritubular de C4d e o infiltrado de linfócitos B, em especial o padrão nodular, estão associados a uma evolução clínica desfavorável do transplante renal. Outra conclusão importante é que há uma associação positiva entre os infiltrados de linfócitos B e de plasmócitos com o C4d peritubular, sugerindo um possível papel destas células responsáveis pela produção de anticorpos na ativação do sistema complemento in situ. Finalmente, as técnicas de IH-criostato e IF-parafina podem ser consideradas técnicas alternativas à técnica de IF-criostato para a detecção do C4d / Allograft rejection mediated by cellular or humoral mechanisms represents an important complication after kidney transplantation. Capillary C4d deposition was recognized as a specific and independent prognostic marker of antibody mediated rejection. The gold standard technique for C4d detection is the immunofluorescence in cryostat sections. However, this technique involves some operating and costs limitations, particularly in Brazil. In antibody mediated rejection, the analysis of B lymphocytes and plasma cells is of pathogenetic relevance since these cells are responsible for antibody production. Considering that the involvement of B lymphocytes and plasma cells in the rejection process is not clear, in this study the CD20 and CD138 expression in kidney biopsies will be also analyzed. Therefore, the aim of the present study was to analyze the C4d detection by 4 different techniques and the infiltration of B lymphocytes and plasma cells in renal allograft biopsies, correlating these findings with the capillary C4d deposition. One hundred and seven biopsies of 82 renal transplant patients were analyzed. C4d was evaluated by immunofluorescence (IF) and immunohistochemistry (IHC) techniques in frozen and paraffin sections (obtained from the same patients), whereas B-lymphocytes and plasma cells were evaluated by immunohistochemistry in paraffin sections using specific antibodies anti-B Lymphocytes (CD20) and anti-plasma cells (CD138). Regarding the C4d detection, the techniques with higher concordance rate with frozen-IF, considered the gold standard, were the frozen-IHC technique (85.4% of cases showed coincident results, r=0.72; p<0.0001) and the paraffin-IF technique (73%, r=0.59; p=0.0001), whereas the concordance rate in the paraffin-IHC technique was only 51.4% (r=0.35; p=0.03). The clinical follow up analysis demonstrate that C4d positive group was associated with a poor graft survival at 3 years post-diagnosis (67% vs 96% in C4d negative group; p=0.01). The histological analysis of mature B cells (CD20+) infiltrate showed 2 distinct patterns: scattered cells and clusters. The cluster pattern was associated with poor graft survival at 3 years (61% vs 89% in the CD20 negative group; p=0.03; and 61% vs 87% in the CD20+ scattered pattern group; p=0.03). The plasma cells infiltrate was not associated with a worse clinical transplant outcome. The analysis of the capillary C4d and B lymphocytes correlation demonstrate that the number of CD20+ and CD138+ cells was significantly higher in C4d positive cases (CD20+: 155±53 vs 26±7 cells/mm2, respectively; p=0.001; CD138+: 46±22 vs 4±1 cells/mm2, respectively; p=0.002). This study concluded that C4d capillary and mature B cells (clusters pattern) are associated with worse graft survival. Another important conclusion is a positive association between B lymphocytes (mature B cells and plasma cells) and capillary C4d, suggesting a possible role of these cells, responsible for antibodies production, in the in situ complement system activation. Finally, the frozen-IHC and paraffin-IF techniques may be considered alternative to frozen-IF technique for C4d detection

Imuno-histoquímica

Imunofluorescência

Linfócitos B

Plasmócitos

Rejeição de enxerto

Transplante de rim

Via clássica do complemento

B-lymphocytes

Complement pathway classical

Fluorescent antibody technique

Graft rejection

Immunohistochemistry

Kidney transplantation

Plasma cells