The roles of HSV-1 VP16 and ICPO in modulating cellular innate antiviral responses

Hancock, Meaghan H.

January 2010

Thesis (Ph.D.)--University of Alberta, 2010. / A thesis submitted to the Faculty of Graduate Studies and Research in partial fulfillment of the requirements for the degree of Doctor of Philosophy in Virology, Medical Microbiology and Immunology. Title from pdf file main screen (viewed on January 10, 2010). Includes bibliographical references.

Cellular immunity, immune activation and regulation in HIV-1 infected mother-child pairs : what are the determinants of protective immunity.

Moodley-Govender, Eshia S.

01 November 2013

Background: Prevention of Mother-to-child transmission (PMTCT) of human immunodeficiency virus (HIV) remains a significant challenge in resource-poor settings despite the advances in antiretroviral (ARV) treatment. HIV-1 infected individuals are able to achieve viral control naturally, however the underlying mechanisms of immunological control in children remains poorly understood. This study was conducted from 2006 to 2010 to investigate correlates of immune control in HIV-1 clade C infected mother-child pairs in the absence of ARVs. Genotypic and phenotypic viral characteristics, cellular immune responses to HIV-1 and host genetics were characterized and correlated with clinical markers of disease progression. Materials and Methods: To achieve the objectives of the study, three cohorts of mother-child pairs were investigated. The first cohort included 60 untreated mother-child pairs and a further ten uninfected children as controls. The second cohort comprised of ARV treated pairs (n=60). The third cohort consisted of 374 mothers and 374 children (infected, exposed uninfected, HIV negative). Plasma viral loads and absolute CD4+ T cell counts were routinely performed in all three cohorts. HIV-specific CD8+ T cell responses were analyzed by interferon gamma (IFN-γ) enzyme linked immunosorbent spot (ELISpot) assays. Viral replicative fitness was assessed using a green fluorescent protein reporter cell line (GFP).Multi-parameter flowcytometry allowed for the investigation of T cell regulation, exhaustion and activation using CD127/CD25, TIM-3/PD-1 and HLA-DR/CD38 markers respectively. IL-10 promoter single nucleotide polymorphisms (SNPs) at positions -592 and -1082 were determined by TaqMan allelic discrimination assays. Plasma IL-10 levels were measured using a luminex assay. Results: To describe the CTL responses elicited to various regions of the HIV proteome in HIV-infected treatment naïve children. Sixty children under one year of age in the untreated cohort were analyzed for CTL responses spanning the HIV genome, for which only 30 had detectable responses. There was no significant difference in viral load between respondersand non-responders (p=0.2799). The responders predominantly targeted Nef (49%), Gag (17%) and Env (14%) regions. Markers of T cell exhaustion and regulation and theirrelationship to markers of disease progression, were next investigated as these parameters may explain the inability of T cells to effectively control HIV infection. T cell phenotyping compared treated, untreated and uninfected subgroups. In infected children, CD8+ T cells were significantly higher for both the inhibitory marker TIM-3 (p=0.001) and exhaustion marker PD-1 (p=0.0001) compared to uninfected children. Median expression of TIM-3 was higher on CD8+ T cells (46%) compared to CD4+ T cells (20%). TIM-3 and PD-1 expression on T cells were maintained at high levels over time. The frequency of absolute Tregs (p=0.0225) were found to be significantly higher in untreated compared to treated children. HLA-DR+CD38+ on CD8+ T cells were significantly up-regulated in untreated children compared to treated (p=0.002) and uninfected children (p=0.0177). HLA-DR+CD38+ was also significantly higher in children less than 6 months compared to older children on CD4+ (p=0.0437) and CD8+ T cells (p=0.00276). Interestingly, we observed a significant negative correlation between magnitude of CTL response and CD25+CD127- (p=0.0202; r=-0.7333) as well as HLA-DR+CD38+ (p=0.0408; r=-0.5516) on CD8+ T cells. IL-10 is an important immunoregulatory cytokine that has been shown to affect the outcome of chronic viral infections. IL-10 polymorphisms have previously been associated with IL-10 levels and HIV-1 outcomes in adults. Polymorphisms associated with different levels of IL-10 production and their relationship with transmission, markers of disease progression and immune responses were next investigated in this mother-child HIV transmission setting. Genetic analysis of IL-10 in cohort three revealed that HIV-1 acquisition was not associated with either IL10 -592 (AA/CA vs CC) or IL10 -1082 (AA/AG vs GG) single nucleotide polymorphisms (SNPSs). There was a significant association between IL10 -1082 and HIV-1 transmission (p=0.0012). No correlation was observed between IL10 -592 (p=0.4279) or IL10 -1082 SNPs (p=0.6361) and mortality rates in children. IL10 -592C was associated with an elevated magnitude of IFN-γ CD8+ T cell response compared to IL10 -529A (p=0.0071). We found a significant positive correlation between IL-10 plasma levels and viral loads (p=0.0068; r=0.4759) and the ages of the children (p=0.0312; r=0.1737). Conclusion: CD8+ T cell responses and viral fitness did not explain differences in disease progression in selected HIV-1 untreated clade C transmission pairs. T cell activation and regulatory markers influence CTL immune responses resulting in poor clinical outcome. IL10 -1082 polymorphisms may be used as a predictor of HIV-1 transmission. The association between increased IL-10 plasma levels and high viral loads suggest that IL-10 contributes to immune dysfunction in paediatric HIV-1 infection. This study has extended our understanding of immunological and genetic correlates of mother-to-child transmission and disease outcome in ARV naïve (naturally controlling) and HIV treated infected children. / Thesis (Ph.D.)-University of KwaZulu-Natal, Durban, 2011.

Cellular immunity.

Immune response--Regulation.

HIV antibodies.

HIV-positive women.

HIV-positive children.

HIV infections--Prevention.

Theses--Paediatrics and child health.

Imunidade humoral e celular de crianças com desnutrição crônica semi-internas no centro de recuperação e educação nutricional, CRE Maceió/AL - 2008 / Humoral and cellular immunity in chronic malnourished children semi-interned in the nutritional and education recovery center (CREN), Maceió/AL - 2008

Moreira, Iramirton Figueirêdo

31 August 2009

The World Health Organization defines protein-energy malnutrition as a range of pathological conditions that appear by a deficient supply, transport or use of nutrients by the body s cells causing an essential amino acid deficiency in DNA and RNA synthesis, which can lead to a substantial immune system impairment. The focus of this research was to evaluate humoral and cellular immunity in children suffering from moderate to severe chronic malnutrition. The cross-sectional study was conducted with children 24-59 months old and 29 days, semi-interned at the Nutritional and Education Recovery Center (CREN), Maceió/AL, suffering from chronic malnutrition. At the same time creating a control group using normal similar aged children, randomly selected enrolled elementary school students from the same community. For data collection a standardized questionnaire was administered to children s parents and guardians addressing the history of infectious diseases. Cellular immunity assessment was performed by counting leukocytes and lymphocytes, B lymphocytes and T and delayed hypersensitivity test. Humoral immunity assessment was determined by immunoglobulins IgA, IgG and IgM in serum and IgG antibody by tetanus toxoid. Nutritional status was determined by the height-for-age (H/A) index. Data analysis used parametric and nonparametric statistics with a significance level (p<0.05). Research participants consisted of 68 children, 34 chronically malnourished and 34 well nourished. Among the malnourished 56% were male versus 47% normal weight, and the (H/A) index ranged from -4.61 to -2.02 in malnourished children versus -0.99 to 1.17 in eutrophic children. The history of airway infections, acute diarrhea, mumps and whooping cough was higher among the malnourished, but there was no statistical difference. The number of leukocytes and lymphocytes was significantly higher in malnourished children (p = 0.00). The number of B and T lymphocytes and delayed hypersensitivity test was not statistically different between the two groups. Serum immunoglobulins IgG and IgA were significantly (p = 0.00) higher among malnourished. Among the malnourished children an apparent decrease of 70.5% of IgG antibodies specific for tetanus toxoid versus 41.2% for normal weight (p = 0.01). Conclusion: There was no humoral and cellular immunity impairment in malnourished children but the number of T lymphocytes was lower and the production of IgG antibodies to tetanus toxoid was significantly lower in severely malnourished children. / A Organização Mundial da Saúde define Desnutrição Energético-Protéica como uma gama de condições patológicas que aparece por deficiência de aporte, transporte ou utilização de nutrientes pelas células do organismo provocando uma deficiência de aminoácidos essenciais na síntese de DNA e RNA, que pode levar a um considerável comprometimento do sistema imune. O objetivo do presente estudo foi avaliar a imunidade humoral e celular de crianças com desnutrição crônica moderada e grave. Estudo do tipo transversal realizado com crianças de 24 a 59 meses e 29 dias, semi-internas no Centro de Recuperação e Educação Nutricional, Maceió/AL, portadoras de desnutrição crônica. No mesmo período constituiu-se um grupo controle composto de crianças eutróficas da mesma faixa etária, selecionado aleatoriamente entre os alunos matriculados na escola de ensino fundamental da mesma comunidade. Para coleta de dados foi utilizado um questionário padronizado, aplicado aos pais ou responsáveis, abordando o histórico das crianças sobre doenças infecciosas. A avaliação da imunidade celular foi realizada através da contagem dos leucócitos e linfócitos totais, linfócitos B e T, e do teste de hipersensibilidade tardia. Para avaliar a imunidade humoral foi feita a determinação das imunoglobulinas IgA, IgG e IgM séricas, e anticorpo do tipo IgG para toxóide tetânico. O estado nutricional foi determinado pelo índice altura para idade (A/I). Na análise dos dados utilizou-se estatística paramétrica e não-paramétrica com nível de significância (p<0,05). Participaram do estudo 68 crianças, sendo 34 desnutridas crônicas e 34 eutróficas. Entre os desnutridos 56% eram do sexo masculino versus 47% dos eutróficos; o índice A/I variou de -4,61 a -2,02 nas crianças desnutridas versus -0,99 a 1,17 nas eutróficas. O histórico de infecções das vias aéreas, diarréia aguda, caxumba e coqueluche foi maior entre os desnutridos, porém não foi observada diferença estatística. O número de leucócitos e linfócitos totais foi significativamente maior nas crianças desnutridas (p = 0,00). O número de linfócitos B e T, e o teste de hipersensibilidade tardia não diferiu estatisticamente entre os dois grupos. As imunoglobulinas séricas IgA e IgG foram significativamente (p = 0,00) mais elevadas entre os desnutridos. Entre as crianças desnutridas 70,5% apresentaram diminuição de anticorpos específicos do tipo IgG para toxóide tetânico versus 41,2% das eutróficas (p = 0,01). Concluiu-se que não houve comprometimento da imunidade celular e humoral nas crianças desnutridas, porém é preciso ressaltar que o número de linfócitos T foi menor e a produção de anticorpos do tipo IgG para toxóide tetânico foi significativamente menor nas crianças desnutridas crônicas.

Protein-energy malnutrition

Humoral immunity

Cellular immunity

Desnutrição energético-protéica

Imunidade humoral

Imunidade celular

CNPQ::CIENCIAS DA SAUDE::NUTRICAO

Respostas mediadas por anticorpos e células T de memória na imunidade contra o Vírus da Bronquite Infecciosa das Galinhas /

Santos, Igor Leonardo dos.

January 2009

Orientador: Hélio José Montassier / Banca: Antonio Carlos Alessi / Banca: Ricardo Luiz Moro de Souza / Banca: Luis Francisco Prata / Banca: Antonio Carlos Paulillo / Resumo: O vírus da bronquite infecciosa aviária (VBIG) permanece como um dos principais problemas para a avicultura industrial. Para a imunoprofilaxia dessa virose existem vacinas "vivas" atenuadas ou inativadas, mas elas não são efetivas para o controle dessa doença infecciosa a longo prazo, especialmente contra estirpes variantes desse vírus. A função primordial das vacinas usuais contra o VBIG são estimular as respostas imunes sistêmicas e locais, mediadas por anticorpos ou por células T efetoras. Com a finalidade de investigar os mecanismos envolvidos na imunidade protetora, os níveis de anticorpos locais e sistêmicos e a expressão de genes associados a respostas de linfócitos T citotóxicos, tais como o CD8 e a granzima A foi avaliada na mucosa traqueal, após a imunização primária de pintinhos de 1 dia de idade com vacinas atenuadas contra o VBIG seguida do desafio 42 dias depois. Proteção ao desafio foi avaliada por meio da ciliostase traqueal, histopatologia e detecção de vírus pela técnica de RT-PCR em tempo real na traquéia. Os níveis de anticorpos no soro e na secreção lacrimal foram mensurados pelo Sandwich- Concanavalina A - ELISA. A expressão dos genes de CD8 e de granzima A foram avaliadas pela técnica de RT-PCR em tempo real. Os resultados demonstraram que a proteção contra a infecção pelo VBIG em aves vacinadas se correlacionou com os níveis de anticorpos anti-virais específicos dos isótipos IgG, IgM e IgA na secreção lacrimal e com os níveis de expressão de CD8 e de granzima A. Concluindo, os resultados possibilataram definir o perfil cinético do desenvolvimento das respostas imunes de memória contra o VBIG na mucosa que é o sítio primário de replicação viral e indicaram que os mecanismos de imunidade humoral e celular podem ser muito importantes para a proteção de hospedeiros naturais contra a infecção pelo VBIG. / Abstract: Avian infectious bronchitis (IBV) remains a major problem in the poultry industry. Live and inactivated vaccines are available, but they are not effective long term in controlling IBV infection, specially against variant strains. The essential function of existing IBV vaccines is to elicit, ideally, local and systemic specific antibodies, as well as cell-mediated immunity to this virus. To investigate the mechanisms of protective immunity, the levels of systemic and local specific antibodies and the expression of genes responsible for cytotoxic T cell killing such as CD8-marker and granzyme-A at tracheal mucosa was evaluated after the primary immunization of 1- day-old chicks with an attenuated avian infectious bronchitis virus (IBV) and challenge 42 days later. Challenge protection was evaluated by tracheal ciliostasis, histopathology and virus detection by real time RT-PCR. The serum and lachrymal anti-IBV antibody levels of IgG, IgM and IgM isotypes were measured with a Sandwich-ELISA Concanavalina-A method. The expression of CD8 and granzyme A genes were evaluated by real time RT-PCR. The results showed protection against challenge with the M-41. Lachrymal IgG, IgM and IgA anti-IBV specific antibodies and the levels of expression of CD8 and granzyme A genes correlated significantly with the protection to challenge. Overall, the results provided the kinetics on the development of memory mucosal immune responses against IBV at the primary replication site and indicate that tracheal humoral and cellular immune mechanisms may be very important in protecting natural hosts against IBV infection. / Mestre

Infecções por coronavírus.

Galinhas.

Vaccine immunity. eng

Immunoglobulin isotypes. eng

Cellular immunity. eng

Tracheal mucosa. eng

Avian coronavirus. eng

Helmintíase intestinal afeta negativamente a resposta celular específica contra o Mycobacterium tuberculosis em pacientes co-infectados

Goulart, Juliana Silva Pancini

27 April 2009

Made available in DSpace on 2016-12-23T13:56:03Z (GMT). No. of bitstreams: 1 HELMINtiASE INTESTINAL.pdf: 1507224 bytes, checksum: 6132aca0f1aadf166d4e2b773c982a74 (MD5) Previous issue date: 2009-04-27 / Mycobacterium tuberculosis (MTB) é um exemplo clássico de patógeno para o qual a resposta protetora depende da imunidade celular do tipo Th1, que é caracterizada pela presença de linfócitos T CD4+ produtores de IFN-g. Essa citocina ativa mecanismos microbicidas no macrófago infectado, levando à eliminação do bacilo. Evidências sugerem que a progressão para a tuberculose esteja relacionada à presença de mecanismos imunossupressores mediados por citocinas e por células T reguladoras. Acredita-se que a presença de helmintíase intestinal possa prejudicar o desenvolvimento de uma resposta adaptativa capaz de conter ou eliminar o MTB, tornando assim o indivíduo susceptível ao adoecimento. Para aquilatar a influência da infecção por helmintos intestinais na resposta celular durante a tuberculose pulmonar, neste trabalho, foram avaliados os perfis quantitativo e fenotípico de populações celulares de sangue periférico e o padrão de citocinas em culturas de sangue total estimuladas com antígenos de MTB, em pacientes portadores de tuberculose pulmonar apresentando ou não helmintíase intestinal no momento do diagnóstico e durante a terapia antituberculose. Para isso, foram arrolados 53 pacientes com diagnóstico recente de tuberculose pulmonar. Desses, 26% eram portadores de pelo menos uma espécie de helminto intestinal. Pacientes com tuberculose pulmonar apresentaram uma redução significativa nos números de linfócitos T CD8+, células NK e NKT. Os indivíduos com helmintíase intestinal associada à tuberculose apresentaram uma maior freqüência de células T reguladoras, com ambos os fenótipos CD4+CD25HIGH e CD4+CD25HIGHFoxp3+. Além disso, os resultados sugerem que a presença de infecção por helmintos intestinais tenha induzido um estado de hipoergia em pacientes portadores de tuberculose pulmonar, uma vez que esses pacientes apresentaram concentrações menores das citocinas IL-2, TNF-a, IL-4, IL-5 e IL-10 nos sobrenadantes de culturas em relação às concentrações encontradas no grupo TB e no grupo controle. Portanto, os resultados desse trabalho sugerem que a presença de infecção por helmintos intestinais tenha um impacto negativo na resposta imunitária à tuberculose em pacientes portadores de tuberculose pulmonar. / The protection against Mycobacterium tuberculosis (MTB) depends on a cellmediated Th1 type-immune response. This response is characterized by IFN-g production by CD4+ T cells, which activates macrophages to enhance microbicidal mechanisms leading to the bacillus eradication. Factors related to tuberculosis resistance or susceptibility are not completely understood. There are evidences suggesting that the progress to active disease is related to immune downregulation caused by suppressors cytokines and regulatory T cells. It is believed that the association with helminth infection can disturb the protective immune response that should contain or eliminate MTB. Here, we investigated the role of intestinal helminth infection on M. tuberculosis specific immune response during active pulmonar tuberculosis in patients with associated tuberculosis and intestinal helminth infection at the time of diagnosis and during tuberculosis therapy. Quantitative and phenotypic analyses of peripheral blood cells populations were performed and the MTBstimulated whole blood culture cytokines production was evaluated. Fifty-three patients with newly diagnosed tuberculosis were enrolled for this study. Twenty-six percent of these patients were infected with at least one intestinal helminth (TB + HELM patients). Patients with pulmonary tuberculosis presented a significant reduction in the numbers of TCD8+, NK and NKT cells. Patients with both intestinal helminth infection and tuberculosis presented higher frequency of regulatory T cells, of both phenotype CD4+CD25HIGH and CD4+CD25HIGHFoxp3+, as compared to TB group, to HELM group, and to control group. In addition, the results suggest a hipoergy status in TB + HELM patients because the production of the cytokines IL-2, TNF-a, IL-4, IL-5 and IL-10 decreased in whole blood culture of these patients as compared to both TB patients and healthy controls. The data from this study indicated that the associated intestinal helminth infection has a negative impact on immunity to tuberculosis in patients with tuberculosis.

tuberculose

helmintíase intestinal

imunidade celular

tuberculosis

intestinal helminth infection

cellular immunity

Respostas mediadas por anticorpos e células T de memória na imunidade contra o Vírus da Bronquite Infecciosa das Galinhas

Santos, Igor Leonardo dos [UNESP]

14 July 2009

Made available in DSpace on 2014-06-11T19:27:58Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-07-14Bitstream added on 2014-06-13T20:36:40Z : No. of bitstreams: 1 santos_il_me_jabo.pdf: 445425 bytes, checksum: 8eabdcdd56ae9af7bcf160cad345bd86 (MD5) / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) / O vírus da bronquite infecciosa aviária (VBIG) permanece como um dos principais problemas para a avicultura industrial. Para a imunoprofilaxia dessa virose existem vacinas “vivas” atenuadas ou inativadas, mas elas não são efetivas para o controle dessa doença infecciosa a longo prazo, especialmente contra estirpes variantes desse vírus. A função primordial das vacinas usuais contra o VBIG são estimular as respostas imunes sistêmicas e locais, mediadas por anticorpos ou por células T efetoras. Com a finalidade de investigar os mecanismos envolvidos na imunidade protetora, os níveis de anticorpos locais e sistêmicos e a expressão de genes associados a respostas de linfócitos T citotóxicos, tais como o CD8 e a granzima A foi avaliada na mucosa traqueal, após a imunização primária de pintinhos de 1 dia de idade com vacinas atenuadas contra o VBIG seguida do desafio 42 dias depois. Proteção ao desafio foi avaliada por meio da ciliostase traqueal, histopatologia e detecção de vírus pela técnica de RT-PCR em tempo real na traquéia. Os níveis de anticorpos no soro e na secreção lacrimal foram mensurados pelo Sandwich- Concanavalina A – ELISA. A expressão dos genes de CD8 e de granzima A foram avaliadas pela técnica de RT-PCR em tempo real. Os resultados demonstraram que a proteção contra a infecção pelo VBIG em aves vacinadas se correlacionou com os níveis de anticorpos anti-virais específicos dos isótipos IgG, IgM e IgA na secreção lacrimal e com os níveis de expressão de CD8 e de granzima A. Concluindo, os resultados possibilataram definir o perfil cinético do desenvolvimento das respostas imunes de memória contra o VBIG na mucosa que é o sítio primário de replicação viral e indicaram que os mecanismos de imunidade humoral e celular podem ser muito importantes para a proteção de hospedeiros naturais contra a infecção pelo VBIG. / Avian infectious bronchitis (IBV) remains a major problem in the poultry industry. Live and inactivated vaccines are available, but they are not effective long term in controlling IBV infection, specially against variant strains. The essential function of existing IBV vaccines is to elicit, ideally, local and systemic specific antibodies, as well as cell-mediated immunity to this virus. To investigate the mechanisms of protective immunity, the levels of systemic and local specific antibodies and the expression of genes responsible for cytotoxic T cell killing such as CD8-marker and granzyme-A at tracheal mucosa was evaluated after the primary immunization of 1- day-old chicks with an attenuated avian infectious bronchitis virus (IBV) and challenge 42 days later. Challenge protection was evaluated by tracheal ciliostasis, histopathology and virus detection by real time RT-PCR. The serum and lachrymal anti-IBV antibody levels of IgG, IgM and IgM isotypes were measured with a Sandwich-ELISA Concanavalina-A method. The expression of CD8 and granzyme A genes were evaluated by real time RT-PCR. The results showed protection against challenge with the M-41. Lachrymal IgG, IgM and IgA anti-IBV specific antibodies and the levels of expression of CD8 and granzyme A genes correlated significantly with the protection to challenge. Overall, the results provided the kinetics on the development of memory mucosal immune responses against IBV at the primary replication site and indicate that tracheal humoral and cellular immune mechanisms may be very important in protecting natural hosts against IBV infection.

Infecções por coronavírus

Galinha

Imunidade vacinal

Imunidade celular

Isótipos de imunoglobulinas

Vaccine immunity

Immunoglobulin isotypes

Cellular immunity

Tracheal mucosa

Avian coronavirus

Aspectos imunológicos do caramujo Pomacea lineata (Spix, 1827) sob condições de estivação induzida

SILVA, Bárbara Brooklyn Timóteo Nascimento

21 February 2014

Submitted by (edna.saturno@ufrpe.br) on 2016-07-19T13:52:24Z No. of bitstreams: 1 Barbara Brooklyn Timoteo Nascimento Silva.pdf: 534821 bytes, checksum: 10562bfdf804ec2c27773d76d75cefab (MD5) / Made available in DSpace on 2016-07-19T13:52:24Z (GMT). No. of bitstreams: 1 Barbara Brooklyn Timoteo Nascimento Silva.pdf: 534821 bytes, checksum: 10562bfdf804ec2c27773d76d75cefab (MD5) Previous issue date: 2014-02-21 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES / Pomacea lineata (Spix, 1827) is a pulmonate gastropod that has a large dependence on humidity, Ampullaridae belongs to the family whose geographic distribution includes almost all the Neotropical Region , which inhabits waters of course slow and stagnate. Pulmonate gastropods have a conspicuous ecological feature, aestivation, which is a form of resistance and adaptation probably best defined as a survival strategy to cope with the arid conditions, but is also typically associated with lack of food availability, and often with high ambient temperatures. During these periods of aestivation some physiological aspects can be changed, as in molluscs, most of these is temperature dependent and can be altered by its variation, including the activity of the immune system. The innate immune system of invertebrates involves humoral and cellular response similar to that found in vertebrates. The cellular defenses occurs in combination with humoral defenses. Humoral responses include the production of reactive oxygen species (ROS) and nitric oxide (NO) and phenol oxidase enzyme activity, and cellular immune reactions are performed by hemocytes, performing, among other functions, encapsulation and phagocytosis of the pathogen. Thus, this research aimed to obtain information on some immunological parameters snail P. lineata in conditions of induced aestivation. The snails were induced to aestivation through the gradual withdrawal of water in the aquarium and abstention from food, getting in these conditions for 60 days. After this period, hemolymph of 40 individuals were collected for analysis of the total haemocyte count, measurement of nitric oxide, phenol oxidase activity and total protein. The results revealed that animals under aestivation showed a significant increase in the total number of hemocytes and measurement of nitric oxide, which may confer greater chance of survival. / Pomacea lineata (Spix, 1827) é um gastrópode pulmonado que apresenta uma grande dependência da umidade, pertencente à família Ampullaridae cuja distribuição geográfica inclui quase toda a Região Neotropical, na qual habita águas de curso lento e estagnadas. Gastrópodes pulmonados apresentam uma característica ecológica conspícua, a estivação, que é uma forma de resistência e adaptação provavelmente melhor definida como uma estratégia de sobrevivência para lidar com as condições áridas, mas também é tipicamente associada com a falta de disponibilidade de alimentos e, frequentemente, com as altas temperaturas ambientais. Durante estes períodos de estivação alguns aspectos fisiológicos podem ser alterados, pois nos moluscos, a maioria desses, é dependente da temperatura e podem ser alterados pela sua variação, incluindo a atividade do sistema imunitário. O sistema imunológico inato dos invertebrados envolve a resposta celular e humoral similarmente ao encontrado nos vertebrados. As defesas celulares ocorrem em combinação com as defesas humorais. As respostas humorais, incluem a produção de espécies reativas de oxigênio (ROS) e óxido nítrico (NO) e a atividade da enzima fenoloxidase, e as reações imunes celulares são realizadas pelos hemócitos, que executam, dentre outras funções, o encapsulamento e fagocitose do patógeno. Assim, esta pesquisa teve por objetivo obter informações sobre alguns parâmetros imunológicos do caramujo P. lineata em condições de estivação induzida. Os caramujos foram induzidos à estivação através da retirada gradual de água no aquário e abstenção de alimento, ficando nestas condições por 60 dias. Após este período, hemolinfa de 40 indivíduos foram coletadas para as análises de contagem total de hemócitos, dosagem de óxido nítrico, atividade da fenoloxidase e proteínas totais. Os resultados revelaram que os animais estivantes apresentavam um aumento significativo no número total de hemócitos e na dosagem de óxido nítrico, o que pode conferir maior chance de sobrevivência.

Estivação

Pomacea lineata

Gastropóda

Hemolinfa

Imunidade celular

Imunidade humoral

Aestivation

Hemolymph

Cellular immunity

Humoral immunity

CIENCIAS AGRARIAS::MEDICINA VETERINARIA

An integrin required for the encapsulation immune response in the tobacco hornworm, Manduca sexta L. (Lepidoptera: Sphingidae).

Levin, David Michael

January 1900

Doctor of Philosophy / Department of Entomology / Michael R. Kanost / James R. Nechols / Cellular encapsulation is the immune response in which insects protect themselves from multicellular parasites such as nematodes or parasitoids. During an encapsulation episode, certain insect hemocytes become attracted to a foreign invader and aggregate on its surface. In short order, the invading entity will become entrapped within a capsule comprised of thousands of hemocytes, thus rendering the parasite harmless to the insect host. Although the process of cellular encapsulation has been known for a great many years, very little knowledge yet exists regarding the biochemistry underlying capsule formation. It would seem likely that cell surface adhesion proteins mediate this immune response. In a series of in vivo encapsulation assays in the tobacco hornworm, Manduca sexta, a collection of anti-hemocyte monoclonal antibodies (mAbs) was screened for their ability to inhibit cellular encapsulation. Two of the mAbs that inhibited this immune response and incidentally specifically bind plasmatocytes, MS13 and MS34, were used to isolate a ≈ 90 kDa protein. Several short peptide sequences contained within this protein were acquired via Edman degradation. Degenerate primers based on two of these peptide sequences and total RNA from M. sexta hemocytes were used to perform RT-PCR and 5´ and 3´ RACE. This resulted in a full-length cDNA sequence of 2426 bp. A 2301 bp open reading frame within this cDNA sequence codes for a protein of 767 residues. This protein, denominated [Beta]Ms1, exhibits significant sequence homology to the [Beta]-subunits of integrins, which are a family of transmembrane, heterodimeric glycoproteins that possess adhesive properties. Analysis of recombinant segments of [Beta]Ms1 showed that the protein produced from the PCR product is the antigen to MS13 and MS34 and that these mAbs bind to the region of the integrin that contains the extracellular binding site. Northern blot analysis of various M. sexta tissues together with immunofluorescence labeling with MS13 and MS34 shows that [Beta]Ms1 is solely expressed in plasmatocytes. The totality of these experiments demonstrates that integrins are essential for the cellular immune response of encapsulation.

encapsulation

integrin

Manduca sexta

insect cellular immunity

hemocyte

cell adhesion

Biology, Cell (0379)

Biology, Entomology (0353)

Chemistry, Biochemistry (0487)

Cellular Immunity in Recombinant Adeno-Associated Virus Vector Mediated Gene Therapy

Xu, Dan

19 October 2011

No description available.

Biomedical Research

Immunology

Molecular Biology

Virology

AAV

gene therapy

viral vector

T-cell immunity

cellular immunity

antigen presentation

Avaliação de potencial agente vacinal contra o S.pyogenes em camundongos transgênicos, portadores de genes HLA de classe II humanos / Evaluation of potential vaccinal agent against s. pyogenes in human HLA class II transgenics mice

Silva, Milton Thiago Guerino da

29 August 2011

A faringite estreptocócica desencadeada pelo Streptococcus pyogenes pode resultar em uma série de doenças humanas e complicações como a febre reumática (FR) em indivíduos predispostos não tratados. A FR é uma doença autoimune que afeta mais de 20 milhões de crianças em países em desenvolvimento. A proteína M presente na membrana do S. pyogenes representa o maior fator de virulência da bactéria, e é objetivo de estudos para o desenvolvimento de uma vacina contra essa patologia. Atualmente mais de 200 tipos de proteínas M foram descritos na literatura e a sua porção Cterminal é conservada entre os diferentes tipos. Desenvolvemos um protótipo de vacina que compreende 55 resíduos de aminoácido da porção C-terminal, denominado StreptInCor. Neste trabalho analisamos a resposta humoral e celular específica contra o peptídeo sintético StreptInCor, usando camundongos transgênicos portadores de HLA de classe II humanos DR2, DR4, DQ6 e DQ8. O protocolo de imunização consistiu em administrar 50 g do StreptInCor adsorvido em 300 g de hidróxido de alumínio nos dias 0 e 14. Os grupos controles foram injetados com salina nas mesmas condições. O soro obtido no 28º dia foi testado por ensaio imunoenzimático (ELISA) para verificarmos a presença de anticorpos contra o StreptInCor e os esplenócitos destes animais, obtidos nessa data, foram utilizados para ensaios de proliferação celular na presença do StreptInCor. Testes de segurança foram efetuados e não observamos reação cruzada contra a miosina cardíaca e após 12 meses de acompanhamento, amostras de tecidos desses animais foram submetidas à análise histológica. Em conclusão não verificamos indícios de reações autoimunes nos animais imunizados com o StreptInCor e os resultados obtidos mostram a capacidade do StreptInCor em desencadear uma resposta imune, duradoura e segura em camundongos portadores de moléculas HLA de classe II / Streptococcal pharyngitis triggered by Streptococcus pyogenes throat infection can result in rheumatic fever (RF) and rheumatic heart disease (RHD) in untreated susceptible individuals. RF is an autoimmune disease that affects more than 20 million children in developing countries. M protein is the major factor of virulence of the bacteria, and it has been studied to develop a vaccine. Currently more than 200 M protein types have been described and its Cterminal domain is conserved in many different serotypes. We developed a vaccine epitope (StreptInCor) composed by 55 amino acid residues of the Cterminal portion of the M protein. In the present work we analyze the ability of the StreptInCor of induce immune response in HLA class II transgenic mice. The transgenic mice harboring the HLA Class II DR2, DR4, DQ6 and DQ8 were immunized subcutaneously with 50 g StreptInCor adsorbed onto 300 g of aluminum hydroxide gel on days 0 and 14. Control groups were immunized with vehicle (Saline) in same conditions. The sera were obtained on day 28 and tested by ELISA to verify the presence of antibodies. The specific cellular immune response was evaluated by proliferation assay using splenocytes. No cross reaction with cardiac myosin were observed. Tissue samples from immunized mice followed by 12 months were analyzed in order to verify if StreptInCor induces some histological damage. No autoimmune or deleterious reactions were observed. In conclusion our results indicate that StreptInCor Induces a good and prolonged and safe immune response in HLA class II transgenic mice

Camundongos transgênicos

Cellular immunity

Genes MHC class II

Humoral immunity

Imunidade celular

Imunidade humoral

Streptococcal vaccine

Transgenic mice

Vacinas estreptocócicas