NK cell alloreactivity against KIR-ligand-mismatched HLA-haploidentical tissue derived from HLA haplotype-homozygous iPSCs. / HLAハプロタイプホモ接合型iPS細胞に由来するKIRリガンド不適合HLA半合致組織に対するNK細胞のアロ反応性

Ichise, Hiroshi

24 November 2017

京都大学 / 0048 / 新制・課程博士 / 博士(医科学) / 甲第20758号 / 医科博第81号 / 新制||医科||6(附属図書館) / 京都大学大学院医学研究科医科学専攻 / (主査)教授 江藤 浩之, 教授 三森 経世, 教授 杉田 昌彦 / 学位規則第4条第1項該当 / Doctor of Medical Science / Kyoto University / DFAM

iPS cell

natural killer cell

transplantation

Human Leukocyte Antigen

killer cell immunoglobulin-like receptor

missing-self response

491

The Roles of Complement C4A and C4B Genetic Diversity and HLA DRB1 Variants on Disease Associations with Juvenile Dermatomyositis and Systemic Lupus Erythematosus

Lintner, Katherine E.

29 September 2016

No description available.

Molecular Biology

Immunology

Genetics

autoimmune diseases

systemic lupus erythematosus

juvenile dermatomyositis

complement system

complement C4

human leukocyte antigen region

Étude du rôle du récepteur ALK1 dans l’infiltration leucocytaire dans l’endothélium

Forget, Arthur

08 1900

Le recrutement des leucocytes dans les tissus est un processus courant dans toutes les maladies inflammatoires de l'adulte. Celui-ci est médié par des interactions de haute affinité entre les molécules d'adhésion endothéliales à la surface des vaisseaux sanguins et leurs ligands sur les cellules immunitaires circulantes. Ce processus implique une multitude de molécules telles que ICAM1, VCAM1 et les sélectines pour soutenir la « capture » des cellules immunitaires et leur extravasation à travers les cellules endothéliales vasculaires. Nos résultats préliminaires suggèrent que le récepteur ALK1, exprimé spécifiquement sur les cellules endothéliales, pourrait réguler l'expression de ces molécules d'adhésion. Pour examiner l'impact de la signalisation ALK1 sur le recrutement des cellules immunitaires, nous avons utilisé des lignées de cellules endothéliales siALK1 (HUVECs) traitées avec du lipopolysaccharide (LPS) pour induire un processus inflammatoire. Tout d'abord, l'expression des gènes, examinée par Ampliseq, a montré une diminution significative de l'expression de ICAM1, VCAM1 et E-sélectine dans les HUVECs siALK1 par rapport au contrôle. De plus, l'analyse par cytométrie en flux a démontré que l'expression des protéines d'adhésion augmentent dans les cellules traitées avec du LPS, mais que cet effet est atténué dans les cellules endothéliales dépourvues d'ALK1. De plus, nous avons observé que le p38 phosphorylé, un facteur qui joue un rôle clé dans le processus inflammatoire, est diminué dans les cellules siALK1. Enfin, pour étudier les conséquences fonctionnelles de la délétion d'ALK1 sur les interactions leucocytes/cellules endothéliales, un test d'adhésion en flux est réalisé, dans lequel les leucocytes circulent sur les cellules endothéliales et l'extravasation des cellules immunitaires est observée au microscope. Les résultats ont montré une diminution de l'infiltration des leucocytes dans les HUVECs siALK1 par rapport aux témoins. En conclusion, nos données démontrent qu'ALK1 a un impact majeur sur le recrutement des leucocytes vers l'endothélium par l'expression de protéines d'adhésion ainsi que par la normalisation vasculaire. Ce projet contribue à une meilleure compréhension de l'interaction entre les leucocytes et l'endothélium vasculaire. / Leukocyte recruitment into tissues is a common process in all adult inflammatory diseases. This is mediated by high affinity interactions between endothelial adhesion molecules and their counter receptor ligands on circulating immune cells. This process involves a multitude of molecules such as ICAM1, VCAM1 and selectins to support the "capture’’ of immune cells and their extravasation through vascular endothelial cells. Our preliminary results suggest that ALK1 receptor, expressed specifically on endothelial cells, could regulate the expression of these adhesion molecules. To examine the impact of ALK1 signaling on immune cells recruitment, we used siALK1 endothelial cell lines (HUVECs) treated with LPS (Lipopolysaccharide) to induce an inflammatory process. First, gene expression, examined by Ampliseq, showed a significant decrease in ICAM1, VCAM1 and E-selectin expression in siALK1 HUVECs compared to control. Furthermore, flow cytometry analysis demonstrated that adhesion protein expression increases in control cells treated with LPS, but that this effect is lessened in endothelial cells lacking ALK1. Moreover, we observed that phosphorylated p38, a factor that plays a key role in inflammatory process, is decreased in siAlk1 cells. Finally, to study the functional consequences of ALK1 deletion on leukocyte/endothelial cells interactions, a flow adhesion assay is performed, in which leukocytes circulate on endothelial cells and extravasation of immune cells is observed under a microscope. The results showed decreased leukocyte infiltration in siALK1 HUVECs compared to controls. In conclusion, our data demonstrate that ALK1 has a major impact on leukocyte recruitment to the endothelium through the expression of adhesion proteins and the vascular normalization. This project contributes to a better understanding of the interaction of leukocytes and the vascular endothelium.

Recruitement

Angiogenèse

Normalisation

Bmp9

Inflammation

Leucocyte

Normalization

Leukocyte

Angiogenesis

Alk1

The role of eicosanoids in the human skin's response to ultraviolet radiation

Gledhill, Karl

January 2009

Erythema is a hallmark skin response to excessive ultraviolet radiation (UVR) and is associated with cutaneous inflammation. Both are mediated by inflammatory mediators including nitric oxide (NO), prostaglandin E2 (PGE2) and chemoattractants such as 12-hydroxyeicosatetraenoic acid (12-HETE) leading to vasodilation and increased leukocyte infiltration. The erythematous response is more pronounced in individuals with low basal melanin levels or who fail to respond to UVR with a robust up-regulation of melanogenesis. While melanin production is a key function of melanocytes, these cells can also produce NO and PGE2, and are located in close proximity to the dermal vasculature. It has been hypothesized that melanocytes with poor melanogenic capacity may participate in the inflammatory response to UVR. The aim of this project was to investigate the inflammatory response in the skin of individuals with either skin phototype (SPT) 1 or 4 to UVR. Sixteen normal healthy individuals were selected for study (8 SPT-1 & 8 SPT-4). Buttock skin was investigated by immunohistochemistry for leukocyte subtypes, eicosanoid producing enzymes and NO synthases under basal and UVR-stimulated conditions. In addition primary cultures of epidermal melanocytes (EM) were established from 16 individuals (8 SPT-1 & 8 SPT-4) and assessed for the presence of eicosanoid-producing enzymes, melanogenic enzymes and NO synthases, by immunocytochemistry, Polymerase Chain Reaction and Western Blotting and for the production of the main pro-inflammatory eicosanoid PGE2 by ELISA and Mass Spectrometry. Moreover, the fatty acid composition of cultured melanocytes was assessed by Gas Chromatography. Results showed that individuals with SPT-1 had significantly greater neutrophil infiltration into the epidermis than those with SPT-4 at 24 hrs post-UVR. Moreover, CD3+ lymphocyte infiltration into the dermis was significantly greater in individuals with SPT-4 than those with SPT-1 at 24 and 72 hrs post-UVR. NOS-1, NOS-3, 12-LOX and COX-2 expression were significantly increased in SPT-1 skin, while NOS-2 and 15-LOX were significantly increased in SPT-4 skin. As 12-LOX and COX-2 products are chemoattractive (for neutrophils) and pro-inflammatory respectively these data could explain the greater observed neutrophil infiltration in SPT-1. The 15-LOX product (15-HETE) is anti-inflammatory and may suggest that 15-LOX up-regulation in SPT-4 skin may aid resolution of the sunburn response, which in part may be mediated by CD3+ lymphocytes and a class-switch in eicosanoid production from COX to LOX products. Melanocyte primary cultures surprisingly showed that SPT was not correlated with melanin content or melanogenic enzyme expression/activity suggesting that all melanocytes in vitro contained the necessary cellular machinery to produce melanin. This finding may reflect also their equal treatment under these enriched culture conditions, which may or may not be available to these cells in situ. Moreover, all melanocytes expressed the necessary machinery (PLA2, COX-1, cPGES) to produce PGE2. However, only some cultures did so at baseline and in response to UVR, and this was not correlated with SPT. A positive correlation was found however between expression level of dopachrome tautomerase (DCT) and protection against PGE2 production in response to UVR, which may suggest a novel role for DCT unrelated to melanogenesis. In summary this research project has generated data that highlights differences between the skin of individuals with SPT-1 and those with SPT-4, and may provide evidence that the keratinocyte partner contributes significantly to the SPT-associated response. This research may also suggest DCT as a novel therapeutic target to protect EM from participation in the UVR-associated inflammatory response in skin.

612.7

Comparison of a leukocyte esterase test with endometrial cytology for the diagnosis of subclinical endometritis and correlation with first service pregnancy rate in postpartum Holstein cows

Couto, Gabriel B.

11 1900

L’objectif de la présente étude était d’évaluer un test d’estérase leucocytaire (LE) pour le diagnostic de l’endométrite subclinique chez les vaches Holstein en période postpartum. Les tests effectués à partir d’échantillons provenant soit de l’endomètre (UtLE) ou du col utérin (CxLE) ont été comparés à la cytologie endométriale (CE). Par ailleurs, deux méthodes d’évaluation des lames ont été comparées. Deux cent quatre vingt-cinq vaches Holstein de 5 troupeaux laitiers commerciaux ont été évaluées entre 21 et 47 jours en lait (JEL). Soixante sept vaches ont été diagnostiquées avec une endométrite clinique suite à un examen transrectal et vaginoscopique et ont été exclues de l’étude. Deux cent dix-huit vaches ont eu des prélèvements pour la CE et le test LE. La fonction ovarienne a été déterminée à la palpation transrectale. La banque de données utilisée pour chacune des vaches a été effectuée à partir du logiciel DSA (Dossier de Santé Animale) laitier. Le pourcentage de neutrophiles était significativement corrélé avec les scores de LE utérin et cervical. L’activité de CxLE et UtLE diminuait significativement avec les JEL, mais n’était pas associée au risque de gestation à 90 JEL (n= 186). Le pourcentage de neutrophiles mesuré à la CE entre 32 et 47 JEL était associé significativement au risque de gestation à 90 JEL (n=94, P=0.04). Pour la même période, selon une analyse de survie, les vaches avec >2,6% de neutrophiles à la CE étaient définies comme étant atteintes d’une endométrite subclinique avec une prévalence de 56%. Les résultats indiquent que le test d’estérase utérin ou cervical a une bonne concordance avec le pourcentage de neutrophiles à la CE. Une endométrite subclinique diagnostiquée par cytologie endometriale entre 32 et 47 JEL est associée à une réduction du risque de gestation au premier service. / The point toward this study was to determine the diagnostic test characteristics of the leukocyte esterase activity test for subclinical endometritis in postpartum Holstein dairy cows. The objectives were 1) to compare uterine leukocyte esterase activity and the endometrial cytology (EC), 2) to compare leukocyte esterase activity of the cervix (CxLE) and the uterus (UtLE), 3) Compare two methods of assessing the slides (i.e. an exhaustive method and a rapid method). Two hundred eighty five post partum Holstein cows from 5 commercial dairy herds had a post partum evaluation between 21 and 47 days in milk (DIM). Sixty seven cows where diagnosed with clinical endometritis by transrectal and vaginoscopy examinations and were excluded from the study. Two hundred eighteen cows were enrolled for endometrial cytology and esterase activity test. The ovarian status was determined by transrectal examination. Computerized databank, dairy DSA (Dossier de Santé Animale) indexing all the cows was used to retrieve individual information for analysis. The percentage of neutrophils was significantly correlated with the LE from the uterus and cervix. The LE from cervix and uterus decreased significantly with DIM, however, they were not statistically associated with pregnancy risk at 90 DIM (n=186). Between 32-47 DIM, the percentage of neutrophils and risk of pregnancy at 90 DIM were associated (n=94, P=0.04). For the same period, survival analysis identified cows with > 2.6 % neutrophils on EC as subclinical endometritis cows with a prevalence of 56%. The two methods for assessing the slides were correlated by 81%. Subclinical endometritis diagnosed by endometrial cytology between 32 and 47 DIM was associated with reduced risk of pregnancy at first service.

Endométrite subclinique

Cytologie endométriale

Estérase leucocytaire

Taux de gestation

Subclinical endometritis

Endometrial cytology

Leukocyte esterase

Outils diagnostique et thérapeutique innovants de la dysfonction vasculaire au cours des maladies artérielles périphériques.

Sarlon-Bartoli, Gabrielle

21 November 2012

Les maladies artérielles périphériques athéromateuses sont graves : l'atteinte des troncs supra-aortiques est à risque d'accident vasculaire cérébral et l'atteinte des artères des membres inférieurs est à risque d'amputation et de décès cardiovasculaire. Le développement de stratégies innovantes capables d'optimiser le diagnostic précoce et le traitement de ces maladies est un enjeu considérable.Nous montrons une corrélation entre deux biomarqueurs inflammatoires, les microparticules leucocytaires (MPL) et la lipoprotéine phospholipase A2, et l'instabilité de la plaque carotidienne définie histologiquement, dans une population de patients porteurs d'une sténose carotidienne serrée. Les MPL sont élevées de façon significative et indépendante y compris chez les patients asymptomatiques porteurs d'une sténose carotidienne serrée instable. Ainsi, le taux circulant de MPL aider à sélectionner les meilleurs candidats à une chirurgie carotidienne préventive parmi les patients ayant une sténose carotidienne serrée asymptomatique. Deuxièmement, nous montrons que l'administration ex vivo d'érythropoïétine (EPO) améliore les capacités proangiogéniques des progéniteurs endothéliaux circulants tardifs in vitro et in vivo sur un modèle d'ischémie de patte de souris nude. Ces effets semblent médiés par la sous-unité CD131 du récepteur à l'EPO. Si ces résultats se confirment chez l'homme, l'EPO pourrait être utilisée pour améliorer les capacités de revascularisation des progéniteurs endothéliaux circulants tardifs circulants humains avant réinjection autologue comme produit de thérapie cellulaire chez des patients atteints d'ischémie critique des membres inférieurs. / Atherosclerotic peripheral arterial diseases are frequent and severe. They undertake the functional and vital prognosis of patients: lesions of supra-aortic trunks are at risk of stroke and lesions of lower limb arteries are at risk of amputation and cardiovascular death. The development of innovative strategies that optimize early diagnosis and therapeutic management of these diseases is thus a considerable challenge.In this work, we show a correlation between inflammatory biomarkers, leukocyte microparticles and lipoprotein phospholipase A2, and carotid plaque instability defined histologically, in a population of patients with tight carotid stenosis with or without neurological symptoms. Leukocyte microparticles are elevated significantly and independently including asymptomatic patients with tight unstable carotid stenosis. Thus, the circulating levels of leukocyte microparticles could be a tool in the future to select the best candidates for carotid surgery among patients with asymptomatic carotid stenosis tight.Second, we show that ex vivo administration of erythropoietin improves the proangiogenic capacity of late circulating endothelial progenitor in vitro and in vivo in a mouse model of hindlimb ischemia. These effects appear mediated by CD131 subunit of the receptor for erythropoietin. If these results are confirmed in humans, erythropoietin could be used to improve the revascularization capacity of late circulating endothelial progenitor before reinjection as autologous cell therapy product in patients with critical ischemia of the lower limbs.

Athérosclérose

Microparticule leucocytaire

Plaque carotidienne instable

Thérapie cellulaire

Ischémie critique

Atherosclerosis

Leukocyte microparticle

Estudo das moléculas imunorregulatórias Galectina-1 e Antígeno Leucocitário Humano-G: da construção de ferramentas ao impacto no diabetes autoimune / Study of the immunoregulatory molecules Galectin-1 and Human Leukocyte Antigen-G: from tool development to impact on autoimmune diabetes

Pelá, Flávia Porto

24 April 2017

O diabetes mellitus tipo 1A (DM1) é uma doença crônica caracterizada pela destruição imunológica das células ? do pâncreas e pela incapacidade de seu portador produzir insulina. Nas últimas décadas foram descritos vários aspectos sobre a fisiopatologia do DM1 e identificado um aumento de sua incidência mundial. Entretanto, na literatura há lacunas a serem respondidas envolvendo a etiologia e a imunopatologia desta doença. No presente trabalho, foi analisado o impacto de duas moléculas endógenas imunoregulatórias, Antígeno Leucocitário Humano-G (HLA-G) e Galectina-1 (GAL-1), no DM1 humano e experimental. Para tanto, as formas recombinantes de HLA-G (-G5 e -G6) e seus respectivos anticorpos foram produzidos e/ou bioquimicamente caracterizados. A partir de amostras de pacientes diagnosticados com DM1 ou de indivíduos controle foi feita uma análise comparativa envolvendo o perfil de expressão do HLA-G e da GAL-1 e a identificação de microRNAs (miRNAs) associados a estas duas moléculas. Camundongos Lgals-/- ou não para o gene da GAL-1 foram tratados com estreptozotocina (STZ) para indução do DM1 experimental. As duas formas recombinantes do HLA-G foram produzidas, mas apenas o HLA-G6 foi caracterizado como uma solução polidispersa contendo um componente majoritário (99,2%) com massa molecular de 23.603,766 Da, raio hidrodinâmico de 6,0 ± 2,0 nm e imunoreatividade para diferentes anticorpos anti-HLA-G comerciais ou produzidos no laboratório. Os níveis transcricional e proteico do HLA-G e da GAL-1 não foram diferentes entre os grupos de indivíduos estudados. A análise comparativa de miRNAs mostrou que a elevada indução do miRNA modulador negativo da expressão do HLA-G (hsa-miR-16-5p) nos controles em relação aos pacientes foi a única associação robusta com a patogenia do DM1. Curiosamente, os animais selvagens apresentam maior suscetilibilidade à indução de DM1 por STZ, uma vez que os indicadores desta doença como o grau de insulite, a taxa de migração de linfócitos T CD4 e T CD8 para os linfonodos pancreáticos, o nível de redução de insulina no pâncreas e a taxa glicêmica estavam aumentados nesses animais em relação aos nocautes para GAL-1. Finalmente, este conjunto de resultados sugere que possa ocorrer uma regulação positiva da expressão de transcritos do HLA-G em pacientes com DM1 e que a presença de GAL-1 endógena pode favorecer o DM1 experimental. Estes dados abrem novas perspectivas para o melhor entendimento da imunopatologia do DM-1 / Diabetes Mellitus type 1A (DM1) is a chronic disease characterized by the immune destruction of pancreatic beta cells and by the consequent inability of its bearer to produce insulin. For the last decades, several aspects of the pathophysiology of DM1 were described and an increase on its worldwide incidence has been identified.Nevertheless, there are gaps in the literature related to aspects of its etiology and immunopathology to be filled.In the present work, the impact of two endogenous immunoregulatory molecules, Human Leukocyte Antigen-G (HLA-G) and Galectin-1 (GAL-1), was analyzed on human and experimental DM1.To do so, the recombinant forms of HLA-G (-G5 and - G6) and its respective antibodies were produced and/or biochemically characterized. A comparative analysis involving the expression profile of HLA-G and GAL-1 and the identification of microRNAs (miRNAs) associated with these two molecules was made from samples of patients diagnosed with DM1, or control subjects. Mice deficient or not for the GAL-1 gene were treated with streptozotocin (STZ) for the induction of experimental DM1.Both recombinant forms of HLA-G were produced, but only HLA-G6 was characterized as a polydisperse solution containing a major component (99.2%), with molecular mass of 23,603,766 Da, hydrodynamic radius of 6.0 ± 2.0 nm, and immunoreactivity for different commercial or lab produced anti-HLA-G antibodies HLA-G and GAL-1. The transcriptional and protein levels were not different between the groups of subjects studied. High induction of the negative modulator miRNA expression of HLA-G (hsa-miR-16-5p) in the controls compared to the patients was the only robust association found with the pathogenesis of DM1.Interestingly, wild type animals presented more susceptibility to the induction of DM1 by STZ, once the indicators of this disease such as the degree of insulin, the migration rate of CD4 T and CD8 T lymphocytes to pancreatic lymph nodes, the level of insulin reduction in the pancreas and the glycemic rate were increased in wild type mice (Lgals-1+/+) when compared to GAL-1-knock out mice (Lgals-1-/-). Finally, this set of results suggests that a positive regulation of the expression of HLA-G transcripts may occur in patients with DM1 and that the presence of endogenous GAL-1 may favor the experimental DM1. These data open new perspectives for a better understanding of the immunopathology of DM-1

Antígeno Leucocitário Humano-G (HLA-G)

Diabetes mellitus tipo 1

Galectin-1

Galectina-1

Human Leukocyte Antigen-G (HLA-G)

Immunoregulation

Imunoregulação

Type 1 Diabetes mellitus

Estudo dos efeitos da solução salina hipertônica e do Ringer lactato sobre a resposta da microcirculação mesentérica e a translocação bacteriana em modelo de obstrução intestinal e isquemia em ratos / Study of the effects of hypertonic saline and lactated Ringer´s solutions on mesenteric microcirculatory response and bacterial translocation in a rat model of intestinal obstruction and ischemia

Zanoni, Fernando Luiz

09 September 2010

INTRODUÇÃO: Estudos demonstram que a solução salina hipertônica melhora a hemodinâmica, a microcirculação e modula o sistema imune, atenuando a resposta inflamatória associada ao choque e trauma. Este estudo tem por objetivo avaliar e comparar os efeitos da solução salina hipertônica (NaCl, 7,5%) e do Ringer lactato seguido da ressecção de segmento do intestino necrosado no tratamento da obstrução intestinal e isquemia, através da análise da translocação bacteriana, da disfunção microcirculatória mesentérica, dos distúrbios hemodinâmicos e metabólicos e da disfunção orgânica. MÉTODOS: Ratos Wistar machos (250 300 g) anestesiados (pentobarbital sódico, 50 mg/kg, i.p.) foram submetidos à obstrução intestinal e isquemia (OI, ligadura ao nível do íleo terminal seguida de ligadura de ramos da artéria mesentérica correspondentes à irrigação de 7 10 cm do íleo). Duas horas após os animais foram randomizados em: OI sem tratamento (OI); OI tratado com Ringer lactato (RL, 4 mL/kg, i.v.); e OI tratado com solução salina hipertônica (SH 7,5%, 4 mL/kg, i.v.). Vinte e quatro horas após os procedimentos cirúrgicos iniciais, os ratos obstruídos (OI, RL e SH) foram submetidos à enterectomia. Ratos controles falso-operados (FO) foram submetidos à lapatotomia. Os seguintes parâmetros foram analisados: 1) cultura bacteriana (E. coli) em amostras de linfonodos mesentéricos, fígado, baço e sangue; 2) análise das interações leucócito-endotélio na microcirculação mesentérica por técnica de microscopia intravital; 3) expressão de moléculas de adesão endoteliais (P-selectina e ICAM-1) por imunohistoquímica; 4) quantificação das citocinas e quimiocinas CINC-1 e CINC-2 no soro por enzimaimunoensaio; 5) histologia intestinal; 6) bioquímica sérica; 7) gasometria, hematócrito, lactato, glicose e leucograma; 8) insulina e corticosterona e; 9) sobrevida. RESULTADOS: O tratamento com SH reduziu a bacteremia, a incidência de animais com amostras positivas para E. coli (57%) e a quantidade de colônias bacterianas (p<0,05) comparado ao tratamento com RL ou aos animais não tratados (OI). As interações leucócito-endotélio e a expressão das moléculas de adesão, P-selectina e ICAM-1, reduziram-se após tratamento com SH seguido de enterectomia a valores observados no grupo controle FO (p>0,05). Ambos os tratamentos, SH e RL, associados à enterectomia normalizaram as concentrações séricas de CINC-1 e CINC-2 (p>0,05). Alterações de PaCO2, pH, lactato e glicemia normalizaram-se após o tratamento dos animais com SH ou RL seguido de enterectomia. A hipoinsulinemia registrada nos ratos OI foi prevenida pelo tratamento dos animais com SH ou RL. As concentrações séricas de corticosterona normalizaram-se após tratamento dos animais com SH associado à enterectomia. A magnitude da lesão intestinal, evidenciada por dano da membrana basal, edema, congestão e presença de células inflamatórias, foi menor no grupo tratado com SH comparado ao tratamento com RL, ambos associados à enterectomia. As concentrações de uréia, creatinina e a atividade das enzimas hepáticas normalizaram-se após tratamento com SH e enterectomia. Houve um aumento significativo da sobrevida dos animais (86%, 15 dias) e no ganho de peso corpóreo (p>0,05 vs FO) no grupo tratado com SH seguido de enterectomia. CONCLUSÕES: A estabilização de ratos submetidos à OI com SH associada à enterectomia resultou em aumento significativo da sobrevida dos animais. A SH reduziu a resposta inflamatória local (interações leucócito-endotélio e expressão de moléculas de adesão na microcirculação mesentérica, e lesão intestinal) e sistêmica (concentrações séricas de CINC-1 e CINC-2, disfunção renal e hepática) / BACKGROUND: It has been shown that hypertonic saline solution improve hemodynamics, the microcirculation, and modulate the immune system, attenuating the inflammatory response associated with shock and trauma. The present study aims to investigate and compare the effects of hypertonic saline solution (NaCl, 7.5%) and lactated Ringer´s solution in the treatment of intestinal obstruction and ischemia, analysing the bacterial translocation phenomenon, mesenteric microcirculatory dysfunctions, hemodynamic/metabolic disturbances, and organ dysfunction in a rat model of intestinal obstruction and ischemia (IO) followed by resection of the necrotic small bowel segment. METHODS: Anesthetized (pentobarbital 50 mg/kg, i.p.) male Wistar rats (250-300 g) were submitted to IO (ligature at the level of the terminal ileum, followed by ligation of mesenteric vessels that supply 7 10 cm of the ileal loop). Two hours thereafter animals were randomized into: IO without treatment; IO treated with lactated Ringer´s (LR, 4 ml/kg, i.v.) solution; IO treated with hypertonic saline (HS, 7.5%, 4 mL/kg, i.v.) solution. Twenty-four hours thereafter, IO rats (IO, LR, HS) were submitted to enterectomy. Control Sham-operated rats were submitted to laparotomy only. The following parameters were analysed: 1) bacterial cultures (E. coli) from mesenteric lymph nodes, liver, spleen, and blood samples; 2) analyses of leukocyte-endothelial interactions at the mesenteric microcirculation by intravital microscopy; 3) expression of endothelial adhesion molecules (P-selectin, ICAM-1) by immunohistochemistry; 4) quantification of serum cytokines and chemokines (CINC-1, CINC-2) by enzyme-linked immunosorbent assay; 5) intestinal histology; 6) serum biochemistry; 7) blood gases, hematocrit, lactate, glycemia, white blood cell counts; 8) serum insulin and corticosterone; 9) survival rate. RESULTS: Treatment with HS reduced the number of animals with positive samples for the presence of E. coli (57%) and the number of CFU/g tissue (p<0.05) compared to LR treated rats or IO rats without treatment. Leukocyteendothelial interactions and expression of the adhesion molecules, Pselectin and ICAM-1, were reduced after treatment with HS solution followed by enterectomy. Values attained matched those observed in Sham group (p>0.05). Both treatments, HS and LR associated with enterectomy, reduced serum levels of CINC-1 and CINC-2 to normal values (p>0.05 vs Sham). PaCO2, pH, lactate, and glucose were normalized after treatment of the animals with HS or LR followed by enterectomy. The hypoinsulinemia observed in the IO rats was prevented by treatment of the animals with HS or LR. Corticosterone concentrations were normalized after treatment of the animals with HS associated with enterectomy. The magnitude of the intestinal lesion, characterized by basal membrane injury, edema, congestion, and inflammatory cells, was smaller in the HS group compared to LR group, both treatments associated with enterectomy. Serum urea and creatinine levels, and the activity of hepatic enzymes were normalized after treatment with HS and enterectomy. A significant increase in survival rate (86%, 15 days) and in the body weight gain (p>0.05 vs Sham) were observed after treatment of the animals with HS and enterectomy. CONCLUSIONS: Treatment of the animals with HS solution followed by enterectomy significantly increased the survival rate. HS solution reduced the magnitude of the local inflammatory response (leukocyte-endothelial interactions, and adhesion molecules expression in the mesenteric microcirculation, and the intestinal lesion) and the systemic inflammatory response (CINC-1 and CINC-2 serum levels, renal and hepatic dysfunctions)

Bacterial translocation

Hypertonic saline solution

Interações leucócito-endotélio

Intestinal obstruction

Leukocyte-endothelial interactions

Obstrução intestinal

Sepse

Sepsis

Solução salina hipertônica

Translocação bacteriana

Inibição in vivo das óxido nítrico sintases: efeitos sobre a expressão de moléculas de adesão e secreção de mediadores inflamatórios / In vivo inhibition of nitric oxide synthases: effects on expressions of adhesion molecules and secretion of inflammatory mediators

Hebeda, Cristina Bichels

17 September 2008

Resultados preliminares do nosso grupo de pesquisa demonstraram que a inibição da síntese de NO por período de tempo prolongado reduz o recrutamento de leucócitos para focos inflamatórios, dependente, pelo menos em parte, da inibição da interação leucócito-endotélio e da expressão de L-selectina. 0 presente trabalho visou complementar os estudos sobre os mecanismos envolvidos nesta ação antiinflamatória. Para tanto, ratos Wistar machos (180 a 220g) receberam L-NAME (20mg/Kg; v.o.; 14 dias) ou água pela mesma via e período de tempo. Foi avaliada a atividade das enzimas óxido nítrico sintases (NOS) no tecido cerebral por radioimunoensaio; o recrutamento leucocitário para cavidade peritoneal induzido pelo LPS (5mg/kg, 4 horas); as expressões de moléculas de adesão em leucócitos do sangue circulante, no músculo cremaster e nos sinusóides hepáticos por ensaios de citometria de fluxo ou imunohistoquímica; as expressões gênicas de moleculas de adesão, quantificadas por PCR e a secreção/produção de mediadores inflamatórios em leucócitos por ensaios imunoenzimáticos, reacao de Griess ou quimiluminescência. Os resultados obtidos mostraram que: 1) o tratamento com L-NAME reduziu em torno de 90% a atividade das NOS dependentes de Ca+2 em condições basais ou após estimulação in vivo com LPS; 2) as concentrações de NO no plasma e no peritônio inflamado estavam reduzidos em animais tratados com L-NAME (30% vs. controles); 3) a migração de leucócitos polimorfonucleares (PMN) para o peritônio inflamado estava reduzida em animais tratados com L-NAME (40% vs. controles); 4) as expressões de L-selectina e PECAM-1 em leucócitos circulantes; de PECAM-1 no endotélio do músculo cremaster e de VAP-1 no endotélio dos sinusóides hepáticos e músculo cremaster de animais tratados com L-NAME estavam reduzidas; 5) a redução na expressão de L-selectina foi dependente de inibição de sua síntese; 6) a concentração de IL-10 estava major no soro de animais tratados com L-NAME em relação aos controles; 7) a maior concentração de IL-10 circulante pode refletir a produção desta citocina por leucócitos na circulação, uma vez que a concentração de IL-10 também estava maior no sobrenadante de leucócitos circulantes de animais tratados com L-NAME; 8) concentrações reduzidas de IL-1&#946; e LTB4 foram detectadas nos sobrenadantes de neutrófilos obtidos de animais tratados com L-NAME; 9) macrófagos obtidos de animais tratados com L-NAME produziram maiores concentrações de IL-1&#946;, TNF-&#945; e IL-6, e menores concentrações de IL-10 na ausência de estimulação; na vigência estimulação in vitro com LPS os macrófagos de animais tratados com L-NAME produziram menores concentrações de NO. Em conjunto, os resultados obtidos neste trabalho mostram que o tratamento com L-NAME por período prolongado de tempo inibe a atividade das NOS dependentes de Ca+2 e nesta condição reduz as concentrações de NO circulante e no foco da inflamação, além de inibir a migração de leucócitos para o foco inflamatório, confirmando propriedades pro-inflamatórias do NO. Os mecanismos envolvidos na inibição da migração celular parecem compreender a modulação da expressão e/ou síntese das moléculas de adesão constitutivas expressas em leucócitos e no endotélio, além da modulação da secreção de mediadores pró ou antiinflamatórios em leucócitos circulantes e neutrófilos. Por outro lado, os efeitos do tratamento com L-NAME sobre a secreção de mediadores químicos por macrófagos induzem a secreção destes e corroboram a dualidade dos efeitos do NO no processo de recrutamento celular. / Our previous results have demonstrated that in vivo chronic inhibition of nitric oxide synthesis reduces leukocyte recruitment into inflammatory focus, dependent, at least in part, on impaired leukocyte-endothelial interactions and expression of L-selectin. This study aimed to clarify the mechanisms involved in the reduced leukocyte migration observed in L-NAME-treated rats. For this purpose, male Wistar rats (180-220g) were treated with L-NAME (20 mg/kg, oral route, 14 days, dissolved in drinking water); controls animals received water by the same route and period of time. The effectiveness of L-NAME treatment was investigated by examining the activity of nitric oxide synthases (NOS) in the brain tissue using radioimmunoassay. In addition, effects of L-NAME treatment were evaluated in LPS-induced leukocyte recruitment into peritoneal cavity (5mg/kg, 4 hours); expression of adhesion molecules was determined in circulating leukocytes, cremaster muscle and liver sinusoids by flow cytometry and immunohistochemistry assay; gene expressions of adhesion molecules were quantified by PCR and leukocyte secretion of inflammatory mediators was measured by immunoenzimatics assays, Griess reaction or chemiluminescence. Our results show that: 1) L-NAME treatment reduced, around 90%, Ca+2 - dependent NOS activity in the presence or not of in vivo inflammation; 2) concentrations of NO in the plasma and into inflamed peritoneum were reduced in L-NAME-treated animals (30% vs. control animals); 3) migration of PMN leukocytes into inflammed peritoneum was impaired in L-NAME-treated rats (40% vs. control animals); 4) expressions of L-selectin and PECAM-1 in circulating leukocytes, PECAM-1 in endothelium from cremaster muscle and VAP-1 in endothelium from liver sinusoids and cremaster muscle were reduced in L-NAME-treated rats; 5) decrease in L-selectin expression was dependent on inhibition of its synthesis; 6) concentrations of IL-10 was higher in serum from L-NAME-treated rats in comparison to control rats; 7) these higher concentrations of circulating IL-10 can reflect the production of this cytokine by leukocytes from circulation, as IL-10 levels was greater in the supernatant of circulating leukocytes obtained from L-NAME-treated animals; 8) L-NAME treatment disturbed neutrophils ability to secrete IL-1&#946; e LTB4, since these concentrations were lower in the supernatants of neutrophils from L-NAME-treated animals; 9) in absence of stimulation, macrophages obtained from L-NAME-treated rats produced higher concentrations of IL-1&#946;, TNF-&#945; e IL-6, and lower concentrations of IL-10, whereas in presence of in vitro LPS these cells produced lower concentrations of NO. Taken together, our results show that L-NAME treatment administrated for a prolonged period of time inhibits Ca+2 -dependent NOS activity, and in this condition, reduces concentrations of NO in plasma and into inflammatory focus and decreases leukocyte migration to the inflammatory focus thus confirming pro-inflammatory properties of NO. The mechanisms involved in impaired cellular migration seem to involve the modulation of expression and/or synthesis of constitutive adhesion molecules in leukocytes and endothelium, and to interfere in the secretion of pro or anti inflammatory mediators. On the other hand, actions of NO in secreation of chemical mediators by macrophages induces the production of inflammatory mediators and support the duality of NO in the cellular recruitment process.

Adhesion molecules

Farmacologia

Inflamação (Estudo)

Inflammatory mediators

L-NAME

L-NAME. Leukocyte recruitment

Leucócitos (Análise)

Mediadores inflamatórios

Moléculas de adesão

Nitric oxide

Óxido nítrico

Pharmacology

Recrutamento leucocitário

Molekulare Mechanismen und strukturelle Dynamik der Interaktion des leukozytären Adhäsionsrezeptors L-Selektin mit intrazellulären Liganden

Beceren-Braun, Figen

23 May 2012

Die Wanderung von Leukozyten aus dem Gefäßlumen läuft in einer Kaskade ab, die durch verschiedene Adhäsionsmoleküle vermittelt wird. Dabei wird der erste Kontakt der Leukozyten mit dem Endothel durch die Interaktion von L­Selektin mit seinen endothelialen Sialomucinliganden eingeleitet. Neben seiner Adhäsionsfunktion kann L­Selektin intrazelluläre Signalwege aktivieren und wird, induziert durch intrazelluläre Signale, an seinen cytoplasmatischen Serinresten durch Proteinkinase C (PKC) phosphoryliert. Über die Regulation dieser Serinphosphorylierung von L-Selektin ist nur wenig bekannt. Ziel dieser Arbeit war die Untersuchung der cytoplasmatischen Interaktion von L-Selektin mit dem Proteinphosphatase 2A-Inhibitor PhapII und die Identifizierung noch unbekannter Interaktionspartner der cytoplasmatischen Domäne von L­Selektin. Es konnte gezeigt werden, dass das basische Duplett Lys-365/Arg-366 der cytoplasmatischen Domäne von L-Selektin essentiell für die Bindung von PhapII ist, die über den sauren C­Terminus von PhapII vermittelt wird. In einem Malachitgrün-basierten Phosphataseassay konnte gezeigt werden, dass die cytoplasmatischen Serinreste von L­Selektin durch Protein Phosphatase 2A (PP2A) dephosphoryliert werden. Ferner konnte in Jurkat-Zelllysaten PP2A als ein direkter Interaktionspartner von nicht phosphoryliertem LScyto identifiziert werden. Die Dephosphorylierung von LScyto konnte durch PhapII verhindert werden, was auf eine Regulation der Serinphosphorylierung durch PKC, PP2A und PhapII hindeutet. Mit dem Ziel, die Interaktion von PhapII mit L-Selektin durch Co-Kristallisation zu untersuchen, wurde PhapII rekombinant exprimiert und gereinigt. Mittels chromatographischer Verfahren konnte PhapII als ein Protein mit intrinsischer Unordnung in seiner Sekundärstruktur beschrieben werden. Die Deletion des sauren C-Terminus bzw. die Mutation an Serin-9 von PhapII zeigten einen Einfluss auf die Konformation von PhapII zu einer kompakteren Proteinstruktur hin. / Migration of leukocytes from the lumen occurs in a cascade mediated by different members of adhesion molecules. The first contact of leukocytes to endothelium is initiated by the interaction of L­selectin to its endothelial sialomucin ligands. Besides its role in cell adhesion, L­selectin can induce a set of intracellular signaling pathways and can be a target of serine phosphorylation by protein kinase C (PKC) induced by intracellular signals. But little information on regulation of this serine phosphorylation of L-selectin and therefore regulation of intracellular protein interactions is known. The aim of this thesis was to analyze the cytoplasmic interaction of L-selectin with the inhibitor of protein phosphatise 2A PhapII and searching for other unknown interaction partners of the cytoplasmic domain of L-selectin. Results show that the basic doublet Lys-365/Arg-366 of the cytoplasmic domain of L­selectin (Lscyto) is essential for binding to PhapII which is mediated by the acidic C­terminal tail of PhapII. Using malachite green based assay to detect free phosphate, cytoplasmic serine residues of L­selectin were dephosphorylated by protein phosphatase 2A (PP2A). In addition, it was possible to identify PP2A as a direct interaction partner of the non-phosphorylated domain of L­selectin in Jurkat T cell lysates. The dephosphorylation of Lscyto was prevented by PhapII and points the regulation of serine phosphorylation by PKC, PP2A and PhapII. For analysis of the interaction of PhapII with L-selectin by co-crystallography, PhapII was recombinantly expressed and purified. Using chromatographic techniques PhapII was observed to be a protein with an intrinsic disorder in its secondary structure. Deletion of the acidic C-terminus and in particular mutation of Serine-9 showed an effect on the conformation of PhapII to a globular and compact protein structure.

Signaltransduktion

L­Selektin

Leukozyt

Phosphatase 2A Inhibitor

signaling

L­selectin

leukocyte

phosphatase 2A inhibitor

570 Biowissenschaften, Biologie

32 Biologie

WW 4120

WW 8840

ddc:570