Immunological Response to Clostridium perfringens in Two Genetically Divergent Lines of Chickens as Influenced by Major Histocompatibility Complex (MHC) Genotype

Sumners, Lindsay Hart

28 July 2011

Chickens genetically selected for low (LA) or high (HA) antibody response to sheep red blood cells (SRBC) displayed a correlated change in major histocompatibility complex (MHC), so that LA chickens were 96% B¹³ and HA chickens were 96% B²¹. During a clinical outbreak of necrotic enteritis, B²¹B²¹ genotypes experienced significantly less mortality (6% vs. 13 %) compared to B¹³B¹³ genotypes. A study was carried out to assess immunological differences between LA and HA lines during exposure to Clostridium perfringens. In Experiment 1, chickens were orally gavaged with a low (10⁷ CFU/mL) or high (10⁹ CFU/mL) dose of C. perfringens. In Experiment 2, chickens were orally gavaged with live coccidia oocysts on experiment d 1, followed by 10⁷ CFU/mL C. perfringens on d 5. Unfortunately, establishment of necrotic enteritis infection was unsuccessful in both experiments as evidenced by lack of significant intestinal lesions, as well as no negative effect on bird performance. In an ex vivo study, peripheral blood mononuclear cells (PBMCs) were isolated from each genetic line, cultured, stimulated with LPS (4 h), and exposed to varying concentrations of C. perfringens α-toxin (1, 10, 100, 1000 U/L) for 2 and 4 h. Evaluation of cellular proliferation, percent cytotoxicity and immunological gene expression was carried out in a variety of experiments. Genetic lines were found to be highly divergent in all analyses. / Master of Science

immune response

genetic resistance

necrotic enteritis

Clostridium perfringens

chicken

Phenotypic and functional changes in populations of murine macrophages during tumor growth

Garner, Ronald Earl

January 1986

Four macrophage (Mφ) surface antigens (Ia, Mac-1, -2, and -3) were examined for their association with Mφ regulatory functions. Observations of antigen expression on Mφ derived from normal or tumor-bearing hosts (TBH) showed that changes occurred in the antigen-defined phenotypes of Mφ which evolve during tumor growth. These changes in antigen expression were correlated with notable changes in Mφ immunoregulatory functions. Experiments using only normal host-derived Mφ showed that in the presence of complement (C), monoclonal antibodies (mAb) directed against Mφ could lyse targeted Mφ and that enrichment of the remaining cells provided populations of Mφ that were altered in their regulatory functions. Analysis of mAb-treated Mφ in the absence of C, suggested that the alterations observed in the presence of C were not due to ligand-receptor activation of peritoneal Mφ and that antibodies alone were not altering Mφ viability. When anti-Mac- I, -2, and -3 antibodies, were used to modify accessory cell activity of whole spleen cell (WSC) or splenic adherent cell (SAC) preparations from normal or TBII, differential susceptibilities of the Mφ were noted. Ligand-receptor activation of WSC by anti-Mac-I was observed in normal but not TBH WSC. With C, anti-Mac-I and -3 each reduced normal and TBH WSC proliferation. To evaluate the possible role of different types of SAC in T cell lectin responsiveness, adherent cells were collected and depleted by antibody plus C treatment and added back to normal T cells. Removal of Mac-1⁺ normal host SAC stimulated the supportive accessory function of the remaining SAC. Enhancing accessory cell function diminished after removal of normal host Mac-2⁺ or TBH Mac-1⁺ SAC. In summary, SAC from normal host demonstrated an accessory cell function corresponding to a Mac-1⁻ phenotype, which was either replaced or obscured by the predominance of a Mac-1⁺ phenotype in TBH. Variable Ia antigen expression by Mφ was examined during tumor growth. Tumor growth induced progressive loss of Ia antigen expression on Mφ. TBH splenic Mφ supported Concanavalin A-induced proliferation of syngeneic T cells (Ia antigen-independent) but did not support syngeneic T cell proliferation in the mixed lymphocyte reaction (MLR) (Ia antigen-dependent). Irrespective of tissue source, normal and TBH Mφ differed in their MLR stimulatory capabilities. In general, splenic Mφ preparations were better stimulators of allogeneic T cell blastogenesis in the MLR than thioglycollate-elicited peritoneal Mφ. Expression of Ia antigens by normal but not TBH Mφ were diminished by 24-hr in vitro plating of the peritoneal Mφ. Indomethacin treatment showed Prostaglandin E₂ was not a direct in vitro factor in Ia antigen-mediated reduction of splenic Mφ MLR stimulatory activity. Taken together, this data suggested a loss of Mφ Ia antigen expression, resulting in a decrease in Ia antigen-mediated functional activities during tumor growth. To continue the assessment of Mφ phenotypes and to determine if alterations in Mφ function during tumor growth included changes in the secretion of soluble regulators of T cell activities, anti-Mac-1, -2, and -3 mAb were used to modulate monokine-mediated regulation of T lymphocyte proliferation. The mAb anti-Mac-1, -2, and -3 (plus C) exhibited differential depletion of normal and TBH Mφ. There was a distinct increase in the number of peroxidase-positive Mφ during tumor growth. Peroxidase-positive TBH Mφ were susceptible to C-mediated lysis by anti-Mac-1 and -3 but not anti-Mac-2, whereas no direct relationship was observed among normal host-derived Mφ. Immunofluorescence of mAb-binding showed a decrease in Mac-2⁺ cells in TBH Mφ populations that was accompanied by an increase in Mac-3 expression. Anti-Mac-2 treatment significantly reduced the ability of TBH Mφ to produce a soluble suppressor(s) but did not alter normal host Mφ-derived suppressor production. In contrast, anti-Mac-1 and -3 treatment of normal host Mφ significantly reduced suppressor production but had diminished effects on TBH Mφ. Anti-Ia plus C treatment of splenic or peritoneal Mφ derived from normal or TBH showed that selection of Ia Mφ increased the secretion of PGE and also increased the T cell suppressor activity in Mφ culture supernatants. Collectively, these data suggest that tumor-induced aberrations in immunoregulation can be attributed to differences in Mφ subpopulations which were discriminated by their surface membrane components. / Ph. D.

LD5655.V856 1986.G376

Immune response

Monoclonal antibodies

Macrophages

The ontogeny of the immune response to sheep erythrocytes and resistance to aflatoxins in chickens

Ubosi, Charles Obidigbo

January 1984

Experiments were conducted to study the ontogeny, kinetics, and the influence of aflatoxin B1 on antibody response to sheep erythrocyte (SRBC) antigen in White Leghorn chickens. In the first experiment, chickens from the parental lines and reciprocal crosses between them were fed diets containing graded levels, from 0 to 5697 ppb of aflatoxin B₁. Aflatoxin depressed body weights, feed consumption and feed conversion, with feed conversion being depressed less than either body weight or feed consumption. Although there were no differences among aflatoxin levels for body core temperatures, levels of 1830 ppb and higher caused progressive decreases in surface temperatures. Heterophilia, lymphopenia and reduced liver metabolism were observed at the 5697 ppb level. Although bursa and thymus weights were smaller in the aflatoxin-fed birds, there was no reduction in their SRBC antibody levels. The second experiment was designed to measure primary and secondary antibody response to intravenous immunization of SRBC antigen. Treatments included immunization at the dosage of SRBC antigen under which selection was practiced, and higher and lower concentrations. Although the dosage of primary immunization influenced the magnitude of the secondary response within population-primary dosage correlations between peak primary and secondary antibody response were not different from zero. Differences among populations in antibody levels appeared as early as day 4 and persisted until day 24 post-primary immunization. Yet, the general response patterns were the same for all populations with respective peaks occurring at the same time. The ontogeny of post-hatching production of antibody SRBC antigen and growth of bursa, thymus and spleen were measured in the third experiment. Both parental lines and reciprocal crosses between them reached serological maturity by 14 days of age. By 7 days, there were differences among populations for frequency of responders to SRBC antigen and magnitude of titers, inferring genetic variation for both the event and subsequent levels of antibody production. / Ph. D.

LD5655.V856 1984.U267

Immune response

Aflatoxins

Chickens -- Diseases

Assessment Of Immune Protective Capacity Of The Recombinant Iron-superoxide Dismutase (fesod) From Bordetella Pertussis

Apak, Aycan

01 December 2011

Whooping cough (pertussis) is a highly contagious acute respiratory disease caused by the strict human pathogen Bordetella pertussis, a gram-negative coccobacillus. The worldwide mass-vaccination was started in 1940s and to date, a number of whole-cell (Pw) and acellular pertussis vaccine (Pa) formulations were developed. Yet the current vaccines are incapable of providing sustained, lifelong immunity and eliminating subclinical infections, which pose a threat especially for unimmunized infants as well as adolescents and adults. Thus, finding new protein candidates with high immune protective capacities is necessary to enhance the clinical efficacy of current acellular pertussis (Pa) vaccines. In this study, iron-superoxide dismutase (FeSOD) protein was investigated for its capacity of conferring protectivity as well as stimulating humoral and cellular responses against B. pertussis infection in a mouse model. For this purpose, sodB gene, which encodes iron-superoxide dismutase FeSOD protein, was amplified from the genomic DNA of the universal B. pertussis strain &lsquo / Tohama I&rsquo / and sequentially cloned to pGEM&reg / -T subcloning and pET-28a(+) expression vectors. Afterwards sodb/pET28a(+) construct was introduced to E. coli BL21(DE3) cells and the gene was overexpressed therein via IPTG induction. The expressed FeSOD protein was then purified by affinity chromatography and its previously reported immunogenicity was confirmed by Western blot. After filter-sterilization, the protein was adsorbed to alum [Al(OH)3] adjuvant and introduced to BALB/c twice at three weeks intervals intraperitoneally at a concentration of 20 &mu / g purified FeSOD protein/mouse. Another group of mice were immunized in tandem with heat-inactivated whole-cell suspension of B. pertussis. Ten days after the second immunization, mice were intranasally challenged with the local &lsquo / Saadet&rsquo / strain of B. pertussis. Next the lungs of groups of mice were excised, homogenized and plated as serial dilutions on days 5, 8 and 14 post-challenge, and viable lung CFU counts were carried out. Whole cell immunization conferred complete bacterial clearance following B. pertussis intranasal infection while FeSOD immunization failed to attain such protection. In addition to the protectivity assay, ELISA was performed to assess the humoral (i.e. IgG) immune response triggered upon FeSOD- and whole-cell immunizations and a statistically significant increase in anti-FeSOD IgG production was observed in FeSOD-immunized group. Finally, cellular immune response was tested via cytokine (IFN-&gamma / ) assay, in which spleens of mice were excised, splenocytes were cultured and the level of IFN-&gamma / production upon FeSOD addition to the cultures was measured via ELISA. This test showed that whole-cell immunization triggered IFN-&gamma / production at significant levels while FeSOD-immunization did not / indicating the failure of alum-adsorbed FeSOD immunization in inducing cell-mediated immune response.

QR Vaccines 189-189.5

Avaliação imunoistoquímica da musculatura estriada esquelética em cães com leishmaniose visceral

Gomes, Ana Amélia Domingues [UNESP]

18 February 2009

Made available in DSpace on 2014-06-11T19:23:46Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-02-18Bitstream added on 2014-06-13T19:30:23Z : No. of bitstreams: 1 gomes_aad_me_jabo.pdf: 566624 bytes, checksum: 460e92b269ccf96c5bd806ac86bfd00f (MD5) / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) / A leishmaniose visceral pode ser incluída como uma das causas de miopatia inflamatória em cães, entretanto, pouco se sabe sobre a patogênese da doença no sistema muscular, sendo incriminada muitas vezes apenas à natureza catabólica da enfermidade. O objetivo deste estudo foi avaliar, por meio de imunoistoquímica, a presença de formas amastigotas de Leishmania sp, linfócitos T (CD3+), macrófagos e IgG nos músculos tríceps braquial, extensor carpo radial, bíceps femoral e gastrocnêmio de 23 cães naturalmente acometidos por leishmaniose visceral. Dentre os 92 músculos avaliados,11 (12%) apresentaram marcação antigênica para formas amastigotas de Leishmania sp, 35 (38,1%) para linfócitos T (CD3+), 29 (31,5%) para macrófagos e 14 (12%) para IgG. Os resultados obtidos permitiram concluir que em cães com leishmaniose visceral apresentam imunomarcação para formas amastigotas de Leishmania sp., linfócitos T CD3+, macrófagos e IgG, sugerindo a participação direta do parasito e de uma resposta imune celular e humoral na fisiopatogenia da lesão muscular. / Visceral leishmaniasis may be included as a cause of inflammatory myophathy in dogs, however, little is known about the pathogenesis of the disease in the muscular system, which is frequently associated with the catabolic nature of the illness. The purpose of this study was investigate, through immunohistochemistry, the presence of amastigote forms of Leishmania sp, T lymphocytes (CD3+), macrophages and IgG in the muscle triceps brachial, extensor carpi radialis, biceps femoris and gastrocnemius of 23 dogs with visceral leishmaniasis. Among 92 evaluated muscles, 11 (12%) presented antigenic marking for amastigote forms of Leishmania sp., 35 (38,1%) for T lymphocites (CD3+), 29 (31,5%) for macrophages and 14 (12%) for IgG. The results of the present experiment led to the conclusion that in dogs with visceral leishmaniasis there may be a straight participation of the parasite and of cellular and humoral immune response in the ethiopatogeny of the muscular injury.

Leishmania

Cão

Imunoperoxidase

Miopatia

Resposta imune celular

Resposta imune humoral

Immunoperoxidase

Myophathy

Cellular immune response

Humoral immune response

Immunophenotypic Variation in Neonatal Pigs and Immunomodulating or Anti-allergic Effects of Microbial Treatments

Schmied, Julie

06 May 2013

Due to the intrauterine environment required to maintain pregnancy it may be that neonatal animals are born type-2 immune response (IR) biased, which consequently may increase susceptibility to certain infectious and immune mediated diseases, such as allergy. Recently, the prevalence of both allergic and autoimmune diseases has increased, leading to the development of the hygiene hypothesis. The hypothesis states that lack of early environmental stimulus leading to inappropriate development and bias in IR, may contribute to this increase. The objectives of this thesis, therefore, were to: (a) Determine the IR bias of neonatal pigs. (b) Investigate the effect of heat-killed Escherichia coli, lipopolysaccharide (LPS) and muramyl dipeptide (MDP) on the IR phenotype and the frequency of allergy in pigs sensitized to the egg white allergen ovomucoid (Ovm). (c) Establish IR phenotypes of pigs allergic or clinically tolerant to Ovm. Immune response bias was determined using an established phenotyping protocol and compared between two groups of pigs, (A) and (B). A difference in IR bias was observed. Bias in IR was not consistently towards type-2. Increase in indicators of type-1 IR, were greater in A and the frequency of type-2 IR correlates were greater in B. It’s likely that unidentified environmental variables may have induced this change, although etiology was not pursued. Treatment with heat-killed Escherichia coli, LPS and MDP had an effect on IR bias and frequency of allergy. Muramyl dipeptide-treatments promoted type-2 bias and were associated with increased frequency of allergy. Pre-treatment with E. coli did not affect allergic frequency, but did elicit the production of a relatively balanced allergen-specific IR phenotype. Lipopolysaccharide-pre-treatment was associated with decreased frequency of allergy. Correlates of an allergic IR phenotype in pigs were also established. The measurement of allergen-specific IgG, IgG1 and/or IgE activity and evaluation of late-phase intradermal skin tests were proposed to be useful in identifying allergic IR phenotypes. This thesis emphasizes the importance of considering the potential for variation in IR in terms of pig health and experimental reproducibility. Further, given the physiological similarities of pigs and humans, these findings may be extended to studies of food allergy in humans. / NSERC, OMAFRA, Ontario Pork, AllerGen NCE

Análise imuno-histoquímica e por imunofluorescência da expressão da interleucina 17 em abscessos e granulomas periapicais / Immunohistochemistry and immunofluorescence analysis of interleukin 17 in periapical abscess and granuloma

Ferreira, Luciana Gonçalves Valente

09 December 2013

Abscessos e granulomas periapicais são considerados lesões inflamatórias relacionadas a elementos dentários, com origem em infecções do tecido pulpar e periapical. É pouco conhecido o papel da interleucina 17 (IL-17) nessas lesões, uma citocina que participa ativamente de uma classe de resposta imunológica recentemente descrita, denominada Th17. A resposta Th17 tem sido caracterizada pela produção de IL-17 por linfócitos CD4+ e tem sido associada à instalação e perpetuação do processo inflamatório, bem como a intenso recrutamento de neutrófilos. Este estudo tem como foco investigar a expressão dessa citocina em lesões de abscesso e granuloma periapicais, com a intenção de verificar se há diferenças de expressão entre essas duas lesões, já que a presença de infiltrado neutrofílico difere bastante entre elas. Testes imuno-histoquímicos para IL-17, CD4 (para identificação de linfócitos T CD4+), CD8 (para identificação de linfócitos T CD8+) e elastase (para identificação de células inflamatórias polimorfonucleadas) foram realizados em casos de abscesso (n=25) e granuloma (n=25) periapicais, selecionados do acervo do Serviço de Patologia Cirúrgica da Disciplina de Patologia Bucal da FOUSP. Foi obtida a porcentagem da área de células com expressão positiva para os marcadores citados. Também foi realizada a quantificação de células CD4+/IL-17+ e CD8+/IL-17+ detectadas por imunofluorescência nessas mesmas biópsias. Foram realizados testes estatísticos de Friedman e Mann-Whitney, para se verificarem as diferenças entre as porcentagens de marcação imuno-histoquímica obtidas para o abscesso e o granuloma, bem como teste de correlação de Spearman, para se verificar se havia correlação entre a expressão de IL-17 e os demais marcadores. Nos casos de abscesso periapical, houve expressão intensa de elastase, seguida de IL-17 e CD8, cujas respectivas porcentagens de expressão não diferiram estatisticamente entre si, mas foram significativamente maiores do que a da expressão do CD4 (p<0,0001). No teste de correlação de Spearman, houve correlação positiva significante entre IL-17 e CD8 (rs = 0,5944, p=0,0415), mas não entre IL-17 e elastase e IL-17 e CD4. Na quantificação de células duplamente positivas pela técnica da imunofluorescência houve significantemente mais células CD4+/IL-17+ do que CD8+/IL-17+ (p=0,0250). Nos casos de granuloma periapical, observou-se que a porcentagem de área de marcação do CD4 foi significativamente maior em relação a da elastase (p=0,0055), do CD8 (p=0,0200) e da IL-17 (p=0,0210). Houve correlação positiva significativa entre IL-17 e elastase (rs = 0,5604, p=0,0463), mas não entre IL-17 e os demais marcadores. Na quantificação de células duplamente positivas pela técnica da imunofluorescência houve significância maior para células CD4+/IL-17 do que de células CD8+/IL-17+ (p=0,0470). Na comparação da porcentagem de área de marcação entre abscesso e granuloma, a porcentagem de IL-17 foi significativamente maior nos abscessos (p=0,0114). Concluiu-se que há maior expressão da IL-17 em abscessos do que em granulomas e que, nesses últimos, essa citocina é mais expressa quando há maior expressão de células polimorfonucleadas. Isso parece evidenciar a participação da resposta Th17 em fases agudas do processo inflamatório. Apesar de haver diferenças significativas entre as lesões quanto ao predomínio das subpopulações de linfócitos T, em ambas as lesões há maior co-expressão da IL-17 em linfócitos CD4+, indicando que provavelmente essa população linfocitária seja a principal responsável pela secreção dessa citocina nas lesões estudadas. / Periapical abscess and periapical granulomas are considered inflammatory lesions related to dental infections originated from pulpal and periodontal tissues. There is little information about the role of interleukin 17 (IL-17) on these lesions. IL-17 is a cytokine pertaining to a new class of immunological response termed Th17. Th17 response has been characterized by the IL-17 release by CD4+ lymphocytes and has been associated to stabilization and perpetuation of the inflammatory process, as well as to neutrophil recruitment. The present study focused on the investigation of the IL-17 expression in periapical abscess and periapical granuloma, in order to verify if there are differences between the lesions that could be related to level of neutrophil infiltrate. Immunohistochemical tests to IL-17, CD4 and CD8 (to identify different lymphocyte population) and elastase (to detect neutrophils) were performed in the periapical abscess (n=25) and granuloma (n=25) biopsies, selected from the collection of Surgical Pathology Service of the Department of Oral Pathology FOUSP. Percentage of the labeling area showing positive expression was obtained for the all cited markers. Counting of CD4+/IL17+ and CD8+/IL7+ cells detected by immunofluorescence was also performed. Friedman´s and Mann-Whitney non-parametric statistical tests were applied for the labeling area percentages in order to detect the significant differences between abscess and granuloma. Spearman´s correlation test was adopted to verify whether there was a correlation between IL-17 and the other markers. In the periapical abscess biopsies, elastase, IL-17, and CD8 were intensively labeled, with area percentage significantly higher than that observed for CD4 (p<0.0001). By the Spearman correlation test, there was significant positive correlation between IL-17 and CD8 (rs = 0.5944, p=0.0415), but not between IL-17 and elastase, and IL-17 and CD4. In the double staining by immunofluorescence there was significantly more CD4+/IL17+ cells than CD8+/IL17+ cells (p=0.0250). In the periapical granulomas, CD4 labeling area percentage was significantly higher than those for elastase (p=0.0055), CD8 (p=0.0200), and IL-17 (p=0.0210). There was significant positive correlation between IL-17 and elastase (rs = 0.5604, p=0.0463), but not between IL-17 and the other markers. The most frequent double staining cells were CD4+/IL17+ cells in the comparison with CD8+/IL17+ cells (p=0.0114). In conclusion, IL-17 labeling area percentage is higher in the abscess than in the granuloma; in the granulomatous lesions the IL-17 expression is directly proportional to the neutrophil infiltration. These results may indicate that the Th17 response participates to the acute phase of the apical inflammatory process. Although there were significant differences regarding the predominant T lymphocytes types, the co-expression of IL-17 and CD4 in the both inflammatory processes may suggest that this CD4+ lymphocytes are the main responsible for IL-17 release in the analyzed periapical lesions.

Abscesso periapical

Adaptative immune response

Granuloma periapical

Innate immune response

Interleucina 17

Interleukin 17

Periapical abscess

Periapical granuloma

Resposta imunológica adaptativa

Resposta imunológica inata

Mecanismo de geração de resposta imune humoral induzida pelo direcionamento do antígeno MSP119PADRE para duas populações distintas de células dendríticas via receptores DEC205 e DCIR2. / Mechanism of generation of humoral immune response induced by targeting of MSP119PADRE antigen to two different subsets of dendritic cells via DEC205 and DCIR2 receptors.

Sulczewski, Fernando Bandeira

24 November 2017

As células dendríticas (DCs) são células do sistema imune inato que são especializadas na instrução de repostas imunes adaptativas No baço murinho, as DCs convencionais podem ser classificadas em CD8&#945;+ DEC205+ e CD8&#945;- DCIR2+. Anticorpos monoclonais (mAbs) &#945;DEC205 e &#945;DCIR2 (33D1) conjugados a proteínas antigênicas e são utilizados como estratégia de direcionamento de antígenos para as DCs CD8&#945;+ e CD8&#945;-. Foi utilizado o antígeno quimérico MSP119PADRE conjugado aos mAbs &#945;DEC205 e &#945;DCIR2 e o Poly I:C como adjuvante. A montagem da resposta celular e humoral foi analisada 3, 4, 5 e 6 dias após primeira e a segunda As DCS CD8&#945;- são especializadas na instrução de células TFH. Porém, num segundo dose de mAbs há a instrução de uma resposta Th2/Th17. E, o direcionamento de antígenos para DCS CD8&#945;+ induz uma resposta Th1, indicando que essas células são especializadas na instrução desse perfil de resposta auxiliar. Apesar disso, na segunda imunização há a diferenciação de células TFH. / As dendritic cells (DC) are innate immune cells that are specialized to prime adaptive immune cells. In the murine spleen, conventional DCs can be classified into CD8&#945;+ DEC205+ and CD8&#945;-DCIR2+. Monoclonal antibodies (mAbs) &#945;DEC205 and &#945;DCIR2 (33D1) conjugated to antigenic proteins have benn used as antigen targeting strategy to CD8&#945;+ and CD8&#945;- DCs. MSP119PADRE chimeric antigen conjugated to mAbs &#945;DEC205 and &#945;DCIR2 and Poly I: C as adjuvant was used. The assembly of the cellular and humoral response was analyzed 3, 4, 5 and 6 days after the first and second doses of imnunization. DCs CD8&#945;- are specialized in the instruction of TFH cells. However, there is an a promotion of Th1 response by CD8&#945;+, indicating that these cells are specialized in the instruction of the helper response profile. Nevertheless, in the second immunization there is a differentiation of TFH cells.

Antigen targeting

Cellular immune response

Células dendríticas

DC subsets

Dendritic cell

Direcionamento de antígenos

Humoral immune response

Resposta imune celular

Resposta imune humoral

Subtipos de DCs

Caracterização das funções dos linfócitos T CD4+ e T CD8+ na cromoblastomicose experimental / Characterization of the functions of CD4+ T lymphocytes and T CD8+ in experimental chromoblastomycosis

Sousa, Maria da Gloria Teixeira de

14 September 2005

A cromoblastomicose é uma infecção fúngica subcutânea causada por fungos da família Dematiceae sendo o principal agente etiológico o fungo Fonsecaea pedrosoi (F. pedrosoi). Estes fungos induzem uma lesão crônica na pele de freqüente recidivas. O objetivo do trabalho foi avaliar alguns aspectos imunológicos na cromoblastomicose experimental através de dois modelos de infecção pelas vias: intraperitoneal (i.p.) e subcutânea (s.c.). No primeiro modelo de infecção pela via s.c. em camundongos BALB/c infectados com 106 conídios de F. pedrosoi, ocorreu a cura espontânea da infecção em aproximadamente 4 semanas. Na subtipagem de linfócitos T em linfonodos regionais ocorreu um predomínio de células T CD4+ que foi constante até a 4ª semana de infecção, no entanto, observamos aumento significativo de linfócitos T CD8+ ao longo da infecção sugerindo que essa população tenha também uma importante participação no controle da doença. Os ensaios de linfoproliferação demonstraram, na 1ª semana de infecção, elevado índice de proliferação celular quando as células de linfonodos foram estimuladas in vitro com antígenos de F. pedrosoi, além da liberação principalmente da citocina IFN-&#947;, já na 4ª semana de infecção não foi detectado proliferação celular. Esses resultados sugerem que no início da infecção a resposta celular seja mediada principalmente por linfócitos T CD4+ produtores de IFN-&#947;, o que nos sugere, que neste modelo experimental, polarize uma resposta de células T do tipo Th1. No segundo modelo de infecção, via intraperitoneal (i.p.), camundongos BALB/c infectados com 106 conídios de F. pedrosoi mostraram desenvolvimento de infecção crônica com preservação da imunidade celular mesmo após a 8ª semana. Ainda pela via i.p., os camundongos C57BL/6 nocautes de T CD4+ apresentaram uma maior carga fúngica no início da infecção e em tempos mais tardios a carga fúngica foi semelhante aos camundongos controles (C57BL/6); esses mesmos animais nocautes não apresentaram uma ativação da resposta celular medida pelo teste de HTT (Hipersensibilidade do Tipo Tardio). Quando avaliamos o padrão de citocinas, a citocina IFN-&#947; produzida pelos órgãos baço e fígado apresentou menores níveis no início da infecção quando comparado ao camundongos controle. Já os níveis de IL-10 aumentaram gradativamente ao longo da infecção e IL-4 não apresentou diferenças em relação ao controle. Nos camundongos nocautes para coa (C57BL/6 CD8 \"KO\"), a carga fúngica, os níveis de citocinas e o teste de HTT foram semelhantes aos animais controle. Esses resultados mostraram que pela via i.p. os linfócitos T, principalmente células T CD4+ são importantes no controle inicial da infecção. Em tempos mais tardios a infecção foi controlada mesmo em camundongos deficientes de linfócitos TCD 4+ ou T CD8+, sugerido que outras células como macrófagos ou NK, estariam atuando de forma mais efetiva no controle da infecção. / Abstract not available.

Adaptative immune response

Adaptative immune response

Bacterial infections (Experiments)

Chromoblastomycosis (Experiments)

Cromoblastomicose (Experimentos)

Fonsecaea pedrosoi

Fonsecaea pedrosoi

Infecções bacterianas (Experimentos)

Medical mycology

Micologia médica

Análise imuno-histoquímica e por imunofluorescência da expressão da interleucina 17 em abscessos e granulomas periapicais / Immunohistochemistry and immunofluorescence analysis of interleukin 17 in periapical abscess and granuloma

Luciana Gonçalves Valente Ferreira

09 December 2013

Abscessos e granulomas periapicais são considerados lesões inflamatórias relacionadas a elementos dentários, com origem em infecções do tecido pulpar e periapical. É pouco conhecido o papel da interleucina 17 (IL-17) nessas lesões, uma citocina que participa ativamente de uma classe de resposta imunológica recentemente descrita, denominada Th17. A resposta Th17 tem sido caracterizada pela produção de IL-17 por linfócitos CD4+ e tem sido associada à instalação e perpetuação do processo inflamatório, bem como a intenso recrutamento de neutrófilos. Este estudo tem como foco investigar a expressão dessa citocina em lesões de abscesso e granuloma periapicais, com a intenção de verificar se há diferenças de expressão entre essas duas lesões, já que a presença de infiltrado neutrofílico difere bastante entre elas. Testes imuno-histoquímicos para IL-17, CD4 (para identificação de linfócitos T CD4+), CD8 (para identificação de linfócitos T CD8+) e elastase (para identificação de células inflamatórias polimorfonucleadas) foram realizados em casos de abscesso (n=25) e granuloma (n=25) periapicais, selecionados do acervo do Serviço de Patologia Cirúrgica da Disciplina de Patologia Bucal da FOUSP. Foi obtida a porcentagem da área de células com expressão positiva para os marcadores citados. Também foi realizada a quantificação de células CD4+/IL-17+ e CD8+/IL-17+ detectadas por imunofluorescência nessas mesmas biópsias. Foram realizados testes estatísticos de Friedman e Mann-Whitney, para se verificarem as diferenças entre as porcentagens de marcação imuno-histoquímica obtidas para o abscesso e o granuloma, bem como teste de correlação de Spearman, para se verificar se havia correlação entre a expressão de IL-17 e os demais marcadores. Nos casos de abscesso periapical, houve expressão intensa de elastase, seguida de IL-17 e CD8, cujas respectivas porcentagens de expressão não diferiram estatisticamente entre si, mas foram significativamente maiores do que a da expressão do CD4 (p<0,0001). No teste de correlação de Spearman, houve correlação positiva significante entre IL-17 e CD8 (rs = 0,5944, p=0,0415), mas não entre IL-17 e elastase e IL-17 e CD4. Na quantificação de células duplamente positivas pela técnica da imunofluorescência houve significantemente mais células CD4+/IL-17+ do que CD8+/IL-17+ (p=0,0250). Nos casos de granuloma periapical, observou-se que a porcentagem de área de marcação do CD4 foi significativamente maior em relação a da elastase (p=0,0055), do CD8 (p=0,0200) e da IL-17 (p=0,0210). Houve correlação positiva significativa entre IL-17 e elastase (rs = 0,5604, p=0,0463), mas não entre IL-17 e os demais marcadores. Na quantificação de células duplamente positivas pela técnica da imunofluorescência houve significância maior para células CD4+/IL-17 do que de células CD8+/IL-17+ (p=0,0470). Na comparação da porcentagem de área de marcação entre abscesso e granuloma, a porcentagem de IL-17 foi significativamente maior nos abscessos (p=0,0114). Concluiu-se que há maior expressão da IL-17 em abscessos do que em granulomas e que, nesses últimos, essa citocina é mais expressa quando há maior expressão de células polimorfonucleadas. Isso parece evidenciar a participação da resposta Th17 em fases agudas do processo inflamatório. Apesar de haver diferenças significativas entre as lesões quanto ao predomínio das subpopulações de linfócitos T, em ambas as lesões há maior co-expressão da IL-17 em linfócitos CD4+, indicando que provavelmente essa população linfocitária seja a principal responsável pela secreção dessa citocina nas lesões estudadas. / Periapical abscess and periapical granulomas are considered inflammatory lesions related to dental infections originated from pulpal and periodontal tissues. There is little information about the role of interleukin 17 (IL-17) on these lesions. IL-17 is a cytokine pertaining to a new class of immunological response termed Th17. Th17 response has been characterized by the IL-17 release by CD4+ lymphocytes and has been associated to stabilization and perpetuation of the inflammatory process, as well as to neutrophil recruitment. The present study focused on the investigation of the IL-17 expression in periapical abscess and periapical granuloma, in order to verify if there are differences between the lesions that could be related to level of neutrophil infiltrate. Immunohistochemical tests to IL-17, CD4 and CD8 (to identify different lymphocyte population) and elastase (to detect neutrophils) were performed in the periapical abscess (n=25) and granuloma (n=25) biopsies, selected from the collection of Surgical Pathology Service of the Department of Oral Pathology FOUSP. Percentage of the labeling area showing positive expression was obtained for the all cited markers. Counting of CD4+/IL17+ and CD8+/IL7+ cells detected by immunofluorescence was also performed. Friedman´s and Mann-Whitney non-parametric statistical tests were applied for the labeling area percentages in order to detect the significant differences between abscess and granuloma. Spearman´s correlation test was adopted to verify whether there was a correlation between IL-17 and the other markers. In the periapical abscess biopsies, elastase, IL-17, and CD8 were intensively labeled, with area percentage significantly higher than that observed for CD4 (p<0.0001). By the Spearman correlation test, there was significant positive correlation between IL-17 and CD8 (rs = 0.5944, p=0.0415), but not between IL-17 and elastase, and IL-17 and CD4. In the double staining by immunofluorescence there was significantly more CD4+/IL17+ cells than CD8+/IL17+ cells (p=0.0250). In the periapical granulomas, CD4 labeling area percentage was significantly higher than those for elastase (p=0.0055), CD8 (p=0.0200), and IL-17 (p=0.0210). There was significant positive correlation between IL-17 and elastase (rs = 0.5604, p=0.0463), but not between IL-17 and the other markers. The most frequent double staining cells were CD4+/IL17+ cells in the comparison with CD8+/IL17+ cells (p=0.0114). In conclusion, IL-17 labeling area percentage is higher in the abscess than in the granuloma; in the granulomatous lesions the IL-17 expression is directly proportional to the neutrophil infiltration. These results may indicate that the Th17 response participates to the acute phase of the apical inflammatory process. Although there were significant differences regarding the predominant T lymphocytes types, the co-expression of IL-17 and CD4 in the both inflammatory processes may suggest that this CD4+ lymphocytes are the main responsible for IL-17 release in the analyzed periapical lesions.

Abscesso periapical

Granuloma periapical

Interleucina 17

Resposta imunológica adaptativa

Resposta imunológica inata

Adaptative immune response

Innate immune response

Interleukin 17

Periapical abscess

Periapical granuloma