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141	Low dose radiation response in the lungs and spleen Muise, Stacy January 2017 (has links) Patients in the intensive and critical care unit frequently undergo diagnostic radiology procedures such as computed tomography (CT) and X-ray imaging. As these patients often require respiratory assistance and are vulnerable to infection, it is important to understand the potential acute effects of these procedures on the lungs and immune system. The aim of this study was to determine the acute effects of a single clinically relevant low-dose X-ray exposure in order to establish baseline responses in markers of lung injury and immune function in a rodent model. Male Sprague-Dawley rats (200-250 g) were irradiated with 0, 2, 20 or 200 mGy whole-body X-rays in an XRAD 320 irradiator. Markers of lung injury and immune activation in the lungs and spleen were evaluated 0.5, 4, and 24 h post-irradiation to examine the acute stages of the physiological and immunological response. Intratrachaeal lipopolysaccharide (LPS) exposure was used as a positive control model of acute lung injury. Lung injury endpoints included respiratory mechanics, pulmonary oedema, arterial blood oxygenation, histological analysis, and cellular and proteinaceous infiltrate via bronchoalveolar lavage. Immunological measures in the spleen focused on splenocyte proliferation, using the MTS assay and differential cell counts before and after stimulation with LPS or concanavalin A (Con A), as compared to unstimulated cultures. Splenocyte proliferation in response to Con A, but not LPS, was significantly decreased after 200 mGy in vivo X-irradiation (repeated measures two-way ANOVA with LSD post-hoc, p=0.024). There was a non-significant trend towards increased lung tissue resistance after 200 mGy, with no significant effect on pulmonary oedema, cellular or proteinaceous infiltrate, nor other aspects of respiratory mechanics (two-way ANOVA with LSD post-hoc, p>0.05). A clear understanding of these immunological and physiological effects informs the responsible use of medical diagnostic procedures in modern medicine. Establishment of this model for the elucidation of acute immune effects of low-dose radiation will facilitate future work evaluating these parameters in disease models, mimicking patients in intensive care. / Thesis / Master of Science (MSc) / Diagnostic procedures such as computed tomography (CT) and X-ray imaging are a common part of intensive and critical care medicine. Some physicians are concerned that this exposure to diagnostic radiation may negatively affect the health of their patients, who are prone to infection and who often need a machine to breathe for them. In order for doctors to make informed decisions, the possible effects of these levels of radiation must be understood. To improve this understanding, this study looked at the short-term effects of X-ray doses on key organs affected by critical illness, the lungs, and the spleen, which is an important organ of the immune system that helps fight infection. Using an animal model, doses of X-rays in the range of diagnostic radiation (0-200 mGy) were examined and no significant effect on lung health was found. However, the highest dose of X-rays tested, which is greater than that expected for a single CT scan, did have an effect on cells from the spleen. Spleen cells are designed to multiply when they detect various types of infection, so that there are more immune cells to fight that infection. The cells from animals that were given the highest dose of X-rays didn’t multiply as much in response to infective stimulus as those from animals that received lower doses, or no X-rays at all. Overall, it seems that diagnostic radiation doesn’t have an effect in the lungs, but very high diagnostic doses could slightly affect a patient’s ability to fight infection. It is important to remember that patients in critical care are very sick, so doctors have good reason to use diagnostic tools available to them. Missing a diagnosis has major and immediate consequences, which must be balanced against the potential small risks of using radiation to make that diagnosis. Read more Radiation biology Immunology Low dose radiation Critical care medicine Lungs Spleen Animal model Rats X-rays Respiratory mechanics
142	Role of Ets-2 in lymphocyte development, function, and survival Fisher, Ian Bradford 22 December 2004 (has links) No description available. Biology, Cell Ets transcription factors Ets-2 Thymus Thymocytes T-lymphocytes Bone marrow Spleen B-lymphocytes Ras MapK Transgenic Mice
143	In Vivo Expansion of Co-Transplanted T Cells Impacts on Tumor Re-Initiating Activity of Human Acute Myeloid Leukemia in NSG Mice Waskow, Claudia, von Bonin, Malte, Wermke, Martin, Nehir Cosgun, Kadriye, Thiede, Christian, Bornhauser, Martin, Wagemaker, Gerard 18 January 2016 (has links) (PDF) Human cells from acute myeloid leukemia (AML) patients are frequently transplanted into immune-compromised mouse strains to provide an in vivo environment for studies on the biology of the disease. Since frequencies of leukemia re-initiating cells are low and a unique cell surface phenotype that includes all tumor re-initiating activity remains unknown, the underlying mechanisms leading to limitations in the xenotransplantation assay need to be understood and overcome to obtain robust engraftment of AML-containing samples. We report here that in the NSG xenotransplantation assay, the large majority of mononucleated cells from patients with AML fail to establish a reproducible myeloid engraftment despite high donor chimerism. Instead, donor-derived cells mainly consist of polyclonal disease-unrelated expanded co-transplanted human T lymphocytes that induce xenogeneic graft versus host disease and mask the engraftment of human AML in mice. Engraftment of mainly myeloid cell types can be enforced by the prevention of T cell expansion through the depletion of lymphocytes from the graft prior transplantation. Blut Knochenmarktransplantation T cells Bone marrow transplantation Bone marrow cells Acute myeloid leukemia White blood cells Blood T cell receptors Spleen ddc:610 rvk:XA 10000
144	La cytokine BAFF et les cellules T CD4+ sont des facteurs de survie majeurs pour les plasmocytes spléniques dans le contexte de déplétion B chez la souris : implications thérapeutiques pour les maladies auto-immunes / BAFF and CD4+ T-cells are major survival factors for long-lived splenic plasma cells in B cell depletion contexts Thai, Lan-Huong 24 October 2016 (has links) L’anticorps monoclonal anti-CD20 (Rituximab) est largement utilisé dans le traitement des maladies auto-immunes. L’analyse de la rate des patients souffrant d’un purpura thrombopénique (PTI) ou d’une anémie hémolytique auto-immune traités par anti-CD20 a mis en évidence que la déplétion lymphocytaire B favorisait la différenciation des plasmocytes (PC) normaux en plasmocytes à longue durée de vie (PLDV) auto-réactifs, expliquant en partie l’absence de réponse à ce traitement. L’enjeu de ce projet a été de savoir si la déplétion lymphocytaire B induit l’émergence de PLDV spléniques et de comprendre les processus impliqués dans la survie plasmocytaire. Pour ce faire, nous avons utilisé le modèle de souris transgénique AID-Cre-ERT2xRosa26-loxP-EYFP qui permet de marquer irréversiblement par la protéine EYFP les cellules B lors de leur passage dans un centre germinatif au cours d’une réponse immune après ingestion de tamoxifène, puis de les suivre in vivo. Les PC EYFP+ ont été générés suite à 2 immunisations avec des globules rouges de mouton. Après avoir sélectionné un set de gènes permettant d’établir les signatures plasmablastiques et plasmocytaires, nous avons comparé par RT-PCR multiplex sur cellules uniques le profil d’expression des PC EYFP+ de la rate de souris traitées ou non par anti-CD20. Nous avons ainsi caractérisé dans le contexte de déplétion B une population plasmocytaire dans la rate homogène et mature, proche des PLDV de la moelle osseuse. Ce profil était différent de celui retrouvé dans la rate des souris contrôles, plus hétérogène, comprenant une majorité de PC intermédiaires entre plasmablastes et PC matures. Nous avons observé le même processus de différenciation paradoxale plasmocytaire dans la rate sous anti-CD20 dans le modèle murin lupique NZB/W, signifiant probablement un mécanisme général, que ce soit en contexte auto-immun ou non, chez l’homme et chez la souris. Nous avons identifié le BAFF (B-cell activating factor) comme un facteur essentiel dans le processus de survie des PC de la rate dans le contexte de déplétion B. En effet, le taux de BAFF augmente dans le sérum et le tissu splénique après traitement par anti-CD20, la combinaison in vivo des traitements anti-CD20 et anti-BAFF induit une diminution drastique des PLDV de la rate, sans générer d’hypogammaglobulinémie IgG. Les granuleux Gr1+ et en particulier les neutrophiles Ly6G+ semblent être la principale source de production de BAFF dans le contexte de déplétion B. Nous avons observé un effet similaire de la combinaison anti-CD20 et anti-BAFF sur les PLDV de la rate dans le modèle lupique NZB/W. Enfin, les LT CD4+ sont un autre composant important de la niche splénique dans le contexte de déplétion B. En effet, le nombre de PC EYFP+ diminue significativement avec l’association anti-CD20 et anti-CD4. Ces résultats suggèrent donc que l’association du traitement anti-CD20 à un inhibiteur de facteur de survie plasmocytaire spécifique de la rate, en particulier BAFF, pourrait avoir un bénéfice clinique au cours des maladies auto-immunes en interférant sur le processus paradoxal de maturation des PC. Un essai clinique associant les traitements anti-CD20 et anti-BAFF au cours du PTI débutera prochainement. / Previous data suggested that the monoclonal anti-CD20 antibody induced paradoxically the settlement of autoreactive splenic long-lived plasma cells (LLPC) in the spleen of patients with auto-immune cytopenia, explaining the treatment failure. To investigate whether this process had a general relevance and decipher its mechanism, we used the AID-CreERT2-EYFP mouse model, which allows the irreversible expression of EYFP in B cells engaged in an immune response after tamoxifen regimen to follow plasma cells at different times after immunization. When analyzed by multiplex PCR at the single-cell level, while the splenic EYFP+B220-PC of untreated mice displayed an intermediate profile between short-lived and long-lived PC, the PC from anti-CD20 treated mice composed a more mature homogeneous population, similar to the long-lived bone marrow PC. The absolute number of splenic EYFP+B220-PC did not change significantly upon anti-CD20 treatment indicating that B-cell depletion promoted PC differentiation rather than a long-lived PC selection. BAFF (B-cell activating factor) and CD4+ T-cells played a major role in plasma cell survival since combination of anti-CD20 with anti-BAFF or anti-CD4 antibodies dramatically reduced the number of splenic EYFP+B220- LLPC. Anti-CD20 treatment also promoted the differentiation of LLPC in the spleen in the lupus prone NZB/W model, while a treatment combining anti-CD20 with anti-BAFF induced a marked reduction in total splenic PC numbers. These results suggest that the process of PC maturation upon anti-CD20 treatment is a general mechanism and that interfering with anti-BAFF antibody at the time of B-cell depletion might greatly improve the response rate in auto-immune disease. Read more Plasmocytes de longue vie Rate Anti-CD20 BAFF Cellules T CD4+ Long-lived plasma cells Spleen Anti-CD20 BAFF CD4+ T cells 616.97
145	Leishmaniose visceral canina: caracterização das alterações histológicas de pele, linfonodo e baço e, a correlação do parasitismo tecidual com a expressão do iNOS / Canine visceral leishmaniasis: characterization of histologic alterations of skin, lymph nodes and spleen, and correlation of tissue parasitism with the expression of iNOS Sanches, Françoise Pereira 21 February 2014 (has links) O presente estudo teve como objetivo caracterizar as alterações histológicas de pele, linfonodo e baço, determinar a densidade de parasitas e de células iNOS+, assim como correlacionar o parasitismo com a expressão de iNOS em pele, baço e linfonodo de cães naturalmente acometidos por leishmaniose visceral. Foram selecionados aleatoriamente, 28 cães infectados com Leishmania (Leishmania) infantum chagasi, oriundos do Centro de Controle de Zoonoses do município de Araçatuba, os quais foram distribuídos em dois grupos, de acordo com sinais clínicos e exames laboratoriais, em sintomáticos (n=18) e assintomáticos (n=10). Um grupo de 6 animais oriundos de área não endêmica para leishmaniose visceral foram empregados como controle negativo. As alterações histológicas de pele foram similares em ambos os grupos clínicos, sintomáticos e assintomáticos, e se caracterizaram por um infiltrado inflamatório na derme, formado por células mononucleares (macrófagos, linfócitos e plasmócitos), que variou de discreto a intenso. No linfonodo, as alterações histológicas foram também semelhantes entre os grupos clínicos, e se caracterizaram por hiperplasia e hipertrofia da área cortical e para-cortical, que variou de discreta a intensa; e por hiperplasia e hipertrofia de macrófagos na região medular, caracterizando em muitos casos uma linfadenite granulomatosa. No baço, alterações histológicas da polpa branca e polpa vermelha foram similares entre os grupos sintomáticos e assintomáticos, com hipoplasia e atrofia de polpa branca e, hipertorfia e hiperplasia de macrófagos na polpa vermelha, variando de moderado a intenso. Quanto ao número de formas amastigotas/mm2 tanto na pele, como no linfonodo e baço, não houve diferença estatisticamente significativa entre os grupos clínicos (p=0,2104), (p=0,2401) e (p=0,8869), respectivamente. Em relação à densidade de células iNOS+(células/mm2), observamos que a infecção por Leishmania levou ao aumento do número destas células na pele, no baço e no linfonodo em relação ao controle (p < 0,05). Porém, quando analisamos a densidade de células iNOS+ entre os grupos clínicos, sintomáticos e assintomáticos, não observamos diferença significativa tanto na pele (p=0,3026), como em linfonodo (p=0,3257) e baço (p=0,5940). Observou-se correlação fraca e não significativa entre a densidade de parasitas e a densidade de células expressando iNOS+ no tegumento; porém no linfonodo, verificou-se correlação negativa moderada e significante (p=0,0034) entre o parasitismo e a expressão de células iNOS+, assim como no baço (p=0,0329), sugerindo que o óxido nítrico deve exercer um papel importante no controle do parasitismo em vísceras / The present study aimed the characterization the histological features in skin, lymph nodes and spleen; determination of the parasitism density and the cells expressing iNOS; and correlation between the parasitism and the expression of iNOS in the skin, lymph nodes and spleen of dogs naturally committed by visceral leishmaniasis. Twenty-eight naturally infected dogs by Leishmania (Leishmania) infantum chagasi were selected randomly from the Zoonosis Control Center of Araçatuba municipality and distributed in two groups according to the clinical signs and laboratory exams, symptomatic (n=18) and asymptomatic (n=10) animals. A group of six animals from non-endemic region for visceral leishmaniais was used as negative control. Histological changes in skin were similar in both clinical groups, symptomatic and asymptomatic, and were characterized by a focal and diffuse inflammatory infiltrate in the dermis of mononuclear cells (macrophages, lymphocytes, plasmocytes), that varied from discrete to intense. In lymph nodes, the histological changes were also similar in both clinical groups, and were characterized by hyperplasia and hypertrophy of the cortical and para-cortical area, that varied from discrete to intense; and hyperplasia and hypertrophy of macrophages in the medullar region characterizing in many cases a granulomatous lymphadenitis. In spleen, the histological alterations in the white pulp and red pulp were similar in both clinical groups, with hypoplasia and hypotrophy of the white pulp and hypertrophy and hyperplasia of macrophages in red pulp varying from moderate to intense. Regarding the results of parasitism density (amastigotes/mm2), we did not observe any significant difference between the clinical groups in skin (p=0.2104), lymph nodes (p=0.2401) and spleen (p=0.8869). Concerning to the density of iNOS+ cells, we observed that the infection by Leishmania caused an increase in the number of these cells in the skin, in spleen and lymph nodes in relation to the control group (p < 0.05). However, when we analyzed the density (cells /mm2) of iNOS+ expressing cells in clinical groups, symptomatic and asymptomatic, we did not observe any significant difference in the skin (p=0.3026), in lymph nodes (p=0.3257) and spleen (p=0.5940). A weak and non-significant correlation was observed between the parasite density and the density of iNOS+ cells in the skin. However, in the lymph node a significant and moderate correlation (p=0.0034) was observed between the parasitism and iNOS+ cells, as well as in the spleen (p=0.0329), suggesting that nitric oxide plays an important role in the control of the parasitism in the viscera Read more Baço Canine visceral leishmaniasis Cellular immunity Histologia Histology Imunidade celular Leishmaniose visceral canina Linfonodo Lymph nodes Nitric oxid Óxido nítrico Pele Skin Spleen
146	Função esplênica e eventos de adesão celular em Anemia Falciforme e em Esferocitose Hereditária / Splenic function and cellular adhesion events in Sickle Cell Anemia and in Hereditary Spherocytosis Ferreira, Priscilla Carnavale Gomes 02 March 2018 (has links) As Anemias Hemolíticas compreendem um grupo de doenças em que há redução acentuada na sobrevivência dos glóbulos vermelhos circulantes e a medula óssea não é capaz de compensação, mesmo aumentando sua produção, o que causa anemia desde os primeiros anos da vida da pessoa. Dentre as doenças deste grupo, a Anemia Falciforme (SCA) e a Esferocitose Hereditária (HS) destacam-se por se tratarem de enfermidades com defeitos genéticos intrínsecos das células vermelhas (RBCs) que geram complicações multissistêmicas agudas e crônicas em seus portadores. Por vias patofisiológicas distintas, reticulócitos e respectivas hemácias defeituosas de tais doenças, falciformes e esferócitos, são continuamente aprisionados e fagocitados no baço, importante órgão de destruição de células velhas e/ou defeituosas via hemólise extravascular, o que leva progressivamente à disfunção e eventual perda da função esplênica. O objetivo desse trabalho é avaliar o papel do baço em relação à habilidade e ao fenótipo adesivos de reticulócitos (ret) e eritrócitos (erit) em pacientes com SCA e HS, com e sem função esplênica preservada. Amostras de sangue de 37 pacientes (22 SCA and 15 HS) com função esplênica e 19 pacientes (13 SCA e 6 HS) sem ela foram avaliadas. Ainda, sangue de 22 crianças com SCA foi coletado em estudo longitudinal dos 6 e 29 meses de vida. Todas as amostras de sangue foram analisadas quanto à função esplênica (Contagem de células PIT e de corpúsculos de Howell-Jolly - HJB), quanto ao perfil imunofenotípico celular (em % e em média de intensidade de fluorescência - MFI) e quanto à habilidade de adesão das células vermelhas à laminina e à linhagem celular endotelial HMEC-1. A análise da transição da perda de função esplênica demonstrou que a mesma se intensificou a partir dos 3 anos de idade (PIT: r=0,8; p<0,0001; HJB: r=0,7; p<0.0001). Quanto à imunofenotipagem celular, a contagem PIT se correlacionou positivamente, principalmente com os marcadores CD147 (%ret: r=0,6; p<0,0001; MFIret: r=0,6; p<0,0001; %erit: r=0,7; p<0,0001; MFIerit: r=0,6; p<0,0001), LuBCAM (%ret: r=0,5; p=0,004; MFIret: r=0,6; p<0,0001; %erit: r=0,6; p<0,0003; MFIerit: r=0,4; p<0,004) and CD58 (%ret: r=0,4; p=0,006; MFIret: r=0,5; p<0,0013; %erit: r=0,4; p<0,009; MFIerit: r=0,6; p<0,0001). Na comparação entre ausência ou presença do baço, a perda de sua função exerceu influência no aumento da expressão de adesão de RBCs em SCA, principalmente CD147 (%ret: p=0,002; MFIret: p=0,003; %erit: p<0,0001; MFIerit: p=0,005), LuBCAM (%ret: p=0,0001; MFIret: p<0,0001; %erit: p<0,0001; MFIerit: p<0,0001) e CD58 (%ret: p=0,007; MFIret: p=0,006; %erit: p=0,003; MFIerit: p=0,0004), embora a adesão celular tenha diminuído em pacientes HS esplenectomizados. Na comparação entre as doenças, pacientes HS com o baço apresentaram maior freqüência de adesão celular em relação aos SCA, notavelmente em relação ao LuBCAM (%ret: p=0,0008; MFIret: p=0,03; %erit: p<0,0001; MFIerit: p=0,0002), CD58 (%ret: p=0,0009; %erit: p=0,003) e CD44 (%ret: p=0,009; %erit: p<0,003). No entanto, as amostras SCA sem função esplênica tiveram maior expressão de adesão celular para CD147 (%ret: p=0,006; MFIret: p=0,02; %erit: p=0,02), LuBCAM (%ret: p=0,004; MFIret: p<0,0001), CD36 (%ret: p=0,0002; MFIret: p=0,01), CD242 (%ret: p=0,0008; %erit: p=0,05) e CD49d (%ret: p=0,04). Em relação ao Ensaio de Adesão in vitro, na ausência de baço, os RBCs SCA apresentaram maior adesividade à laminina do que os RBCs SCA com função esplênica preservadaem todas as taxas de fluxo de tensão de cisalhamento empregadas (0,5 dyne/cm2: p=0,01; 1 dyne/cm2: p=0,02; 2 dynes/cm2: p=0,03; 3 dynes/cm2: p=0,03; 5 dynes/cm2: p=0,04 e 7 dynes/cm2: p=0,03). Especialmente, reticulócitos de pacientes sem baço apresentaram maior adesividade à HMEC-1 em baixas tensões de cisalhamento (1 dyne/cm2) em ambas as doenças (SCA: p=0,03; HS: p=0,03). Por fim, reticulócitos apresentaram maior habilidade adesiva à células endoteliais em indivíduos SCA do que em pacientes HS, com (0,5 dyne/cm2: p=0,04; 1 dyne/cm2: p=0,03) ou sem baço (0,5 dyne/cm2: p=0,02; 2 dynes/cm2: p=0,01; 3 dynes/cm2: p=0,03; 5 dynes/cm2: p=0,02 e 7 dynes/cm2: p=0,03). Nossos resultados indicam que embora pertençam ao grupo de Anemias Hemolíticas, as patofisiologias e evoluções clínicas distintas de SCA e de HS levam a padrões imunofenotípicos diferentes de expressão da adesão celular. Na SCA, a ausência de função esplênica teria direta relação com o aumento do fenótipo pró-adesivo e com a adesividade de RBCs SCA, o que traz sérias consequências clínicas aos pacientes, enquanto na HS sem baço, de maneira geral, os eventos de adesão celular são minimizados, embora ainda apresentem reticulócitos e eritrócitos adesivos circulantes após a esplenectomia. / Hemolytic Anemias comprise a group of diseases in which there is marked reduction in the survival of circulating erythrocytes and the bone marrow is not capable of compensation, even by increasing its production, which causes anemia from the first years of the person\'s life on. Among the diseases of this group, Sickle Cell Anemia (SCA) and Hereditary Spherocytosis (HS) stand out for being diseases with intrinsic genetic defects of red blood cells (RBCs) that generate acute and chronic multisystemic complications in their patients. By distinct pathophysiological pathways, reticulocytes and these disease\'s respective defective erythrocytes, sickle and spheroid ones, are continuously trapped and phagocytosed in the spleen, important organ of destruction of old and/or defective cells via extravascular hemolysis, which progressively leads to dysfunction and eventual loss of splenic function. The objective of this study was to evaluate the role of the spleen in relation to the reticulocyte (ret) and erythrocyte (eryt) adhesive ability and adhesion phenotype in patients with SCA and HS, with and without preserved splenic function. Blood samples from 37 patients (22 SCA and 15 HS) with splenic function and 19 patients (13 SCA and 6 HS) without it were evaluated. Still, blood from 22 children with SCA was collected in a longitudinal study from 6 to 29 months of age. All blood samples were analyzed for splenic function [pitted cells (PIT) and Howell-Jolly bodies (HJB) counting], for the cellular immunophenotypic profile (in % and in mean fluorescence intensity - MFI) and for the adhesive ability of RBCs to laminin and to endothelial cell line HMEC-1. Analysis of the splenic function loss transition showed that it intensified from 3 years of age on (PIT: r=0.8, p<0.0001; HJB: r=0.7, p<0.0001). Regarding the cellular immunophenotyping, PIT count correlated positively, mainly with CD147 markers (%ret: r=0.6, p<0.0001; MFIret: r=0.6, p<0.0001; %eryt: r=0.7, p<0.0001; MFIeryt: r=0.6, p<0.0001), LuBCAM (%ret: r=0.5, p=0.004; MFIret: r=0.6, p<0.0001; %eryt: r=0.6, p<0.0003; MFIeryt: r=0.4, p<0.004) and CD58 (%ret: r=0.4, p=0.006; MFIret: r=0.5, p<0.0013; %eryt: r=0.4, p<0.009; MFIeryt: r=0.6, p<0.0001). In the comparison between spleen absence or presence, the loss of its function exerted influence on the increase of RBCs adhesion expression in SCA, mainly on CD147 (%ret: p=0.002; MFIret: p=0.003; %eryt: p<0.0001; MFIeryt: p=0.005), LuBCAM (%ret: p=0.0001; MFIret: p<0.0001; %eryt: p<0.0001; MFIeryt: p<0.0001) e CD58 (%ret: p=0.007; MFIret: p=0.006; %eryt: p=0.003; MFIeryt: p=0.0004), although cell adhesion has been decreased in splenectomized HS patients. In the comparison between diseases, HS patients with spleen showed higher cell adhesion frequency compared to SCA, notably in relation to LuBCAM (%ret: p=0.0008; MFIret: p=0.03; %eryt: p<0.0001; MFIeryt: p=0.0002), CD58 (%ret: p=0.0009; %eryt: p=0.003) and CD44 (%ret: p=0.009; %eryt: p<0.003). However, SCA samples without splenic function had higher cell adhesion expression for CD147 (%ret: p=0.006; MFIret: p=0.02; %eryt: p=0.02), LuBCAM (%ret: p=0.004; MFIret: p<0.0001), CD36 (%ret: p=0.0002; MFIret: p=0.01), CD242 (%ret: p=0.0008; %eryt: p=0.05) and CD49d (%ret: p=0.04). Concerning the in vitro Adhesion Assay, in the spleen absence, SCA RBCs showed greater adhesiveness to laminin than SCA RBCs with preserved splenic function did at all shear stress flow rates applied (0.5 dyne/cm2: p=0.01, 1 dyne/cm2: p=0.02, 2 dynes/cm2: p=0.03, 3 dynes/cm2: p=0.03, 5 dynes/cm2: p=0.04 and 7 dynes/cm2:p=0.03). Especially, reticulocytes from patients without spleen showed higher adhesiveness to HMEC-1 at low shear stresses (1 dyne/cm2) in both diseases (SCA: p=0.03; HS: p=0.03). Finally, reticulocytes showed greater adhesion ability to endothelial cells in SCA subjects than in HS patients, with (0.5 dyne/cm2: p=0.04 and 1 dyne/cm2: p=0.03) or without spleen (0.5 dyne/cm2: p=0.02, 2 dynes/cm2: p=0.01, 3 dynes/cm2: p=0.03, 5 dynes/cm2: p=0.02 and 7 dynes/cm2: p=0.03). Our results indicate that although both diseases belong to the Hemolytic Anemias group, SCA and HS distinct pathophysiologies and clinical evolution lead to different immunophenotypic patterns of cell adhesion expression. In SCA, the absence of splenic function may have a direct relation with the increase of SCA RBCs proadhesive phenotype and adhesiveness, which brings serious clinical consequences to the patients, whereas in HS without spleen, in general, cellular adhesion events are minimized, although they still present adhesive circulating reticulocytes and erythrocytes after splenectomy. Read more Adesão Celular Anemia Falciforme Baço Cellular Adhesion Esferocitose Hereditária Função Esplênica Hereditary Spherocy Reticulócitos Reticulocytes Sickle Cell Anemia Spleen Splenic Function
147	Leishmaniose visceral canina: caracterização das alterações histológicas de pele, linfonodo e baço e, a correlação do parasitismo tecidual com a expressão do iNOS / Canine visceral leishmaniasis: characterization of histologic alterations of skin, lymph nodes and spleen, and correlation of tissue parasitism with the expression of iNOS Françoise Pereira Sanches 21 February 2014 (has links) O presente estudo teve como objetivo caracterizar as alterações histológicas de pele, linfonodo e baço, determinar a densidade de parasitas e de células iNOS+, assim como correlacionar o parasitismo com a expressão de iNOS em pele, baço e linfonodo de cães naturalmente acometidos por leishmaniose visceral. Foram selecionados aleatoriamente, 28 cães infectados com Leishmania (Leishmania) infantum chagasi, oriundos do Centro de Controle de Zoonoses do município de Araçatuba, os quais foram distribuídos em dois grupos, de acordo com sinais clínicos e exames laboratoriais, em sintomáticos (n=18) e assintomáticos (n=10). Um grupo de 6 animais oriundos de área não endêmica para leishmaniose visceral foram empregados como controle negativo. As alterações histológicas de pele foram similares em ambos os grupos clínicos, sintomáticos e assintomáticos, e se caracterizaram por um infiltrado inflamatório na derme, formado por células mononucleares (macrófagos, linfócitos e plasmócitos), que variou de discreto a intenso. No linfonodo, as alterações histológicas foram também semelhantes entre os grupos clínicos, e se caracterizaram por hiperplasia e hipertrofia da área cortical e para-cortical, que variou de discreta a intensa; e por hiperplasia e hipertrofia de macrófagos na região medular, caracterizando em muitos casos uma linfadenite granulomatosa. No baço, alterações histológicas da polpa branca e polpa vermelha foram similares entre os grupos sintomáticos e assintomáticos, com hipoplasia e atrofia de polpa branca e, hipertorfia e hiperplasia de macrófagos na polpa vermelha, variando de moderado a intenso. Quanto ao número de formas amastigotas/mm2 tanto na pele, como no linfonodo e baço, não houve diferença estatisticamente significativa entre os grupos clínicos (p=0,2104), (p=0,2401) e (p=0,8869), respectivamente. Em relação à densidade de células iNOS+(células/mm2), observamos que a infecção por Leishmania levou ao aumento do número destas células na pele, no baço e no linfonodo em relação ao controle (p < 0,05). Porém, quando analisamos a densidade de células iNOS+ entre os grupos clínicos, sintomáticos e assintomáticos, não observamos diferença significativa tanto na pele (p=0,3026), como em linfonodo (p=0,3257) e baço (p=0,5940). Observou-se correlação fraca e não significativa entre a densidade de parasitas e a densidade de células expressando iNOS+ no tegumento; porém no linfonodo, verificou-se correlação negativa moderada e significante (p=0,0034) entre o parasitismo e a expressão de células iNOS+, assim como no baço (p=0,0329), sugerindo que o óxido nítrico deve exercer um papel importante no controle do parasitismo em vísceras / The present study aimed the characterization the histological features in skin, lymph nodes and spleen; determination of the parasitism density and the cells expressing iNOS; and correlation between the parasitism and the expression of iNOS in the skin, lymph nodes and spleen of dogs naturally committed by visceral leishmaniasis. Twenty-eight naturally infected dogs by Leishmania (Leishmania) infantum chagasi were selected randomly from the Zoonosis Control Center of Araçatuba municipality and distributed in two groups according to the clinical signs and laboratory exams, symptomatic (n=18) and asymptomatic (n=10) animals. A group of six animals from non-endemic region for visceral leishmaniais was used as negative control. Histological changes in skin were similar in both clinical groups, symptomatic and asymptomatic, and were characterized by a focal and diffuse inflammatory infiltrate in the dermis of mononuclear cells (macrophages, lymphocytes, plasmocytes), that varied from discrete to intense. In lymph nodes, the histological changes were also similar in both clinical groups, and were characterized by hyperplasia and hypertrophy of the cortical and para-cortical area, that varied from discrete to intense; and hyperplasia and hypertrophy of macrophages in the medullar region characterizing in many cases a granulomatous lymphadenitis. In spleen, the histological alterations in the white pulp and red pulp were similar in both clinical groups, with hypoplasia and hypotrophy of the white pulp and hypertrophy and hyperplasia of macrophages in red pulp varying from moderate to intense. Regarding the results of parasitism density (amastigotes/mm2), we did not observe any significant difference between the clinical groups in skin (p=0.2104), lymph nodes (p=0.2401) and spleen (p=0.8869). Concerning to the density of iNOS+ cells, we observed that the infection by Leishmania caused an increase in the number of these cells in the skin, in spleen and lymph nodes in relation to the control group (p < 0.05). However, when we analyzed the density (cells /mm2) of iNOS+ expressing cells in clinical groups, symptomatic and asymptomatic, we did not observe any significant difference in the skin (p=0.3026), in lymph nodes (p=0.3257) and spleen (p=0.5940). A weak and non-significant correlation was observed between the parasite density and the density of iNOS+ cells in the skin. However, in the lymph node a significant and moderate correlation (p=0.0034) was observed between the parasitism and iNOS+ cells, as well as in the spleen (p=0.0329), suggesting that nitric oxide plays an important role in the control of the parasitism in the viscera Read more Baço Histologia Imunidade celular Leishmaniose visceral canina Linfonodo Óxido nítrico Pele Canine visceral leishmaniasis Cellular immunity Histology Lymph nodes Nitric oxid Skin Spleen
148	Caracterização do perfil de compostos orgânicos voláteis produzidos por cultura de células e animais infectados com Leishmania infantum / Characterization of the profile of volatile organic compounds produced by cell cultures and animals infected with Leishmania infantum Anchieta, Naira Ferreira 19 December 2016 (has links) Alguns parasitas modificam o perfil de Compostos Orgânicos Voláteis (COVs) de seus hospedeiros na tentativa de atrais/dispersar seus vetores, assegurando a propagação do parasita e a manutenção do ciclo da doença. É sabido que o mosquito Lutzomyia longipalpis, vetor da Leishmaniose Visceral (LV) são mais atraídos por cães infectados que não infectados. Este trabalho tem como objetivo identificar e caracterizar os Compostos Orgânicos Voláteis emitidos por culturas de células e hamsters infectados Mesocricetus auratus com Leishmania infantum (MHOM/74/PP75). Células aderentes mononucleares de baço de hamsters foram separadas com Ficoll e distribuídas em placas de 24 poços com 2x106 células por poço. Após 42 horas, as células foram infectadas e os COVs foram coletados por \"headspace\" por 18 horas. Os COVs foram determinados por comparação com as placas controle: controle células aderentes mononucleares, controle L. infantum, e controle meio RPMI 1640.40 Hamsters foram subdivididos em 2 grupos: 20 animais foram infectados com formas promastigotas metacíclicas de L. infantum selecionadas com aglutinina de amendoim (PNA) por via intracardíaca com 1x107 parasitas. Os animais foram acompanhados por 4 meses pós infecção e as amostras foram coletadas colocando os animais em sacos de poliéster conectados com um tubo de metal recheado com Tenax TA acoplado a uma bomba de sucção automática por 10 minutos. Todas as amostras foram analisadas por dessorção térmica via Cromatografia gasosa/ Espectrometria de Massas (CG-EM). Nas culturas de células, 2 compostos estão presentes apenas nas culturas infectadas: 1,2-difenilciclobutano e (E)-(2,3-Difenil Ciclopropil)-metil-fenilsulfóxido. O 2,4-dimetilbenzaldeído estava presente na placa controle contendo meio RPMI 1640. Por outro lado, em ambas as placas infectadas e controle com células aderentes mononucleares, o 3-metileno-heptano estava presente. Outros compostos contendo os grupos químicos aldeídos ou álcoois ou hidrocarbonetos aromáticos foram detectados em todas as placas, mas com diferentes áreas de pico (quantidade). Quando comparamos os COVs emitidos por hamsters infectados e controles, nenhuma diferença foi encontrada. Os compostos emitidos por culturas de células infectadas mostram que a infecção com L.infantum é capaz de modificar o perfil de COVs em culturas de células. Outros compostos encontrados em todas as placas, mas com diferentes áreas de pico podem indicar que a infecção aumenta a liberação de algumas substâncias que são possíveis atrativos para vetores. / Some parasites can modify their hosts Volatile Organic Compounds (VOCs) profile in order to attract / disperse their vectors, ensuring spreading of the parasite and maintenance of the disease cycle. It is already known that Lutzomyia longipalpis sandflies, the vectors of Visceral Leishmaniasis (VL), are more attracted to infected than to non-infected dogs. This work aims to identify and characterize the VOCs emitted by cell cultures and hamsters Mesocricetus auratus infected with Leishmania infantum (MHOM/74/PP75). Spleen adherent mononuclear cells of hamsters were separed with Ficoll and distributed in flat-bottomed 24-well plates at 2x106 cells per well. After 42 hours, the cells were infected and VOCs were collected from the \"headspace\" for 18 hours. The VOCs were determined in comparison with the controls plates: control mononuclear adherent cells, control L. infantum and control medium RPMI 1640. 40 Hamsters were subdivided in two groups: 20 animals were used as a control group and 20 animals were infected with metaciclic form of L. infantum selected by peanut agglutinin (PNA) by intracardiac route with 1x107 parasites. The animals were followed up for 4 months post-infection and the samples were collected by introducing the hamsters in a polyester bag connected with a metal tube filled with the Tenax TA adsorbent coupled to an automatic suction pump for 10 minutes. All samples were analyzed by thermal desorption via Gas Chromatography/Mass Spectrometry (GCMS). In cell cultures, two compounds were present only in infected cultures: 1, 2- diphenyl cyclobutane, and trans-[(2, 3-Diphenylcyclopropyl) methyl] phenyl sulfoxide. 2, 4-dimethyl benzaldehyde was present in the control well containing RPMI 1640 medium. On the other hand, in both infected and control wells with mononuclear adherent cells, 3-methylene heptane was present. Other compounds containing either aldehydes or alcohols or aromatic hydrocarbon chemical groups were detected in all plates, but with different peak areas (i.e., amounts). When comparing the VOCs emitted by infected and control hamsters, no difference was found. The compounds emitted only by infected cell cultures show that the infection with L. infantum is able to modify the profile of VOCs in cell cultures. The other compounds found in all plates but with different peak areas may indicate that infection may increase the release of some substances that are possible attractants for vectors. Read more Células Aderentes Mononucleares Compostos Orgânicos Voláteis Leishmania infantum Leishmania infantum Lutzomyia longipalpis Volatile Organic Compounds
149	Elastografia hepatoesplênica para predizer varizes esofágicas em pacientes com hipertensão portal não cirrótica: estudo de acurácia diagnóstica / Liver and spleen transient elastography to predict esophageal varices in patients with non-cirrhotic portal hypertension: a diagnostic accuracy study Ramos, Danusa de Souza 17 September 2018 (has links) Introdução: elastografia ultrassônica é um método não invasivo validado e rotineiro para a determinação indireta do grau de fibrose hepática e em investigação para predizer a presença de varizes esofágicas. Entretanto, a elastografia foi validada somente em doenças que evoluem para cirrose. Na revisão de literatura que realizamos, observamos que há escassez de estudos de acurácia diagnóstica em pacientes com hipertensão portal não cirrótica. Objetivos: avaliar a acurácia diagnóstica das técnicas de elastografia hepatoesplênica (transitória por FibroScan e ARFI) para predizer a presença de varizes esofágicas e se as varizes são de risco de sangramento em pacientes com hipertensão portal não cirrótica. Avaliar a concordâncias das duas técnicas e correlacioná-las com outros índices (plaquetas/baço, APRI e FIB-4). Métodos: Foram incluídos pacientes com diagnóstico confirmado das seguintes condições: oclusão da veia porta extra-hepática, esquistossomose mansônica, hipertensão portal não cirrótica idiopática e fibrose hepática congênita. A endoscopia digestiva alta foi considerada como marcador da presença de hipertensão portal clinicamente significante. Critérios de inclusão: idade acima de um ano; diagnóstico etiológico definido; concordância do paciente ou responsável legal em participar do estudo. Critérios de exclusão: cirrose, confirmada pela combinação de critérios diagnósticos clínicos, de imagem e laboratoriais ou pela biópsia hepática quando o resultado estivesse disponível; hipertensão portal pós sinusoidal; condições que impeçam tecnicamente a realização da elastografia (ascite volumosa e insuficiência cardíaca); esplenectomia; gestação; carcinoma hepatocelular avançado. O desenho do estudo foi prospectivo, transversal, de acordo com a metodologia STARD, avaliando a acurácia, sensibilidade, especificidade, valores preditivos positivos e negativos e razões de verossimilhança positiva e negativa. Procedimentos no estudo: consulta aos dados de prontuário; ultrassonografia abdominal e elastografia hepatoesplênica com os equipamentos/métodos FibroScan e ARFI. Os pontos de corte foram determinados por curva ROC. Resultados: os valores de elastografia transitória hepática por FibroScan foram de 5,91 ± 1,87 kPa na oclusão da veia porta extra-hepática, 8,89 ± 3,96 kPa na esquistossomose, 10,60 ± 3,89 kPa na hipertensão portal não cirrótica idiopática e 10,30 ± 4,14 kPa na fibrose hepática congênita, enquanto os valores de ARFI foram de 1,27 ± 0,23 m/s; 1,35 ± 0,45 m/s; 1,43 ± 0,40 m/s; 1,55 ± 0,39 m/s; respectivamente. Os valores de elastografia transitória esplênica por FibroScan foram de 60,82 ± 20,56 kPa na oclusão da veia porta extra-hepática, 54,16 ± 22,94 kPa na esquistossomose, 52,64 kPa ± 21,97 kPa na hipertensão portal não cirrótica idiopática e 48,50 ± 24,86 kPa na fibrose hepática congênita, enquanto os valores de ARFI foram de 3,22 ± 0,62 m/s; 3,01 ± 0,74 m/s; 2,86 ± 0,53 m/s; 2,80 ± 0,55 m/s; respectivamente. A elastografia esplênica por FibroScan com ponto de corte 65,1 kPa apresentou acurácia de 0,62 (intervalo de confiança 95% 0,46-0,78; p=0,121) para presença de varizes. Para predizer varizes de alto risco de sangramento, o melhor ponto de corte foi 40,05 kPa, que apresentou acurácia de 0,63 (intervalo de confiança 95% 0,52-0,76; p=0,016). A elastografia esplênica ARFI com ponto de corte de 2,67m/s apresentou acurácia de 0,64 (intervalo de confiança 95%, 0,50-0,78; p=0,065) para presença de varizes. O melhor ponto de corte para predizer varizes de alto risco de sangramento com esse método foi de 3,17m/s, que apresentou acurácia de 0,61 (intervalo de confiança 95%, 0,51- 0,71; p=0,033). Conclusões: métodos de elastografia esplênica apresentaram uma acurácia moderada e valor preditivo positivo elevado para diagnosticar presença de varizes. A elastografia transitória esplênica por FibroScan quando associada à razão plaqueta/baço apresentou acurácia moderada com especificidade alta para predizer varizes de alto risco de sangramento. Entretanto, considerável superposição de valores foi observada entre pacientes com e sem varizes esofagianas, o que limita a aplicação a utilidade clínica do método / Background and rationale: transient elastography is a noninvasive, validated, method allowing evaluation of liver fibrosis by measurement of liver stiffness and under investigation to predict the presence of esophageal varices. However, elastography has been validated only in diseases that progress to cirrhosis. In a literature review we found few studies on diagnostic accuracy in patients with non-cirrhotic portal hypertension. Aims: to evaluate the accuracy of hepatosplenic elastography (FibroScan and ARFI) to predict the presence of esophageal varices and whether varices are at risk of bleeding in patients with non-cirrhotic portal hypertension. To evaluate the concordances of the two techniques and correlate them with other indexes such as the platelet /spleen diameter ratio, APRI and FIB-4. Methods: patients with confirmed diagnosis of the following conditions were included: extrahepatic portal vein occlusion, schistosomiasis, idiopathic non-cirrhotic portal hypertension and congenital hepatic fibrosis. Upper digestive endoscopy was considered as a marker of the presence of clinically significant portal hypertension. Inclusion criteria: age above one year; defined etiological diagnosis; agreement of the patient or legal guardian to participate in the study. Exclusion criteria: cirrhosis confirmed by combination of clinical, imaging and laboratory diagnostic criteria or by liver biopsy when the result was available; post sinusoidal portal hypertension; conditions that technically preclude the performance of elastography (massive ascites and heart failure); splenectomy; pregnancy; advanced hepatocellular carcinoma. The study design was prospective, transversal, according to the STARD methodology, evaluating the accuracy, sensitivity, specificity, positive and negative predictive values and positive and negative likelihood ratios. The procedures of the study were: review of medical records data, abdominal ultrasonography and hepatosplenic elastography with FibroScan and ARFI equipment / methods. Cut-off points for elastography were determined by ROC curves. Results: liver stiffness measurement by FibroScan were 5.91 ± 1.87 kPa in extrahepatic portal vein occlusion, 8.89 ± 3.96 kPa in schistosomiasis, 10.60 ± 3.89 kPa in portal hypertension non-cirrhotic idiopathic and 10.30 ± 4.14 kPa in congenital hepatic fibrosis, whereas by ARFI were 1.27 ± 0.23 m/s; 1.35 ± 0.45 m/s; 1.43 ± 0.40 m/s; 1.55 ± 0.39 m/s; respectively. Spleen stiffness measurement by FibroScan were 60.82 ± 20.56 kPa in extrahepatic portal vein occlusion, 54.16 ± 22.94 kPa in schistosomiasis, 52.64 ± 21.97 kPa in idiopathic non-cirrhotic portal hypertension, and 48.50 ± 24.86 kPa in congenital hepatic fibrosis, while by ARFI were 3.22 ± 0.62 m/s; 3.01 ± 0.74 m/s; 2.86 ± 0.53 m/s; 2.80 ± 0.55 m/s; respectively. Liver stiffness measurement by FibroScan with a cut-off of 65.1 kPa had an accuracy of 0.62 (95%confidence interval, 0.46-0.78, p=0.121) for the presence of esophageal varices. The best cut-off point for predicting the presence of varices at high risk of bleeding was 40.05 kPa (accuracy, 0.63, 95% confidence interval, 0.52-0.76, p = 0.016). The spleen stiffness measurement by ARFI with a cut-off of 2.67 m/s showed (accuracy, 0.64, 95% confidence interval, 0.50-0.78, p=0.065) for the presence of esophageal varices. The best cut-off point for predicting the presence of varices at high risk of bleeding was 3.17 m/s (accuracy, 0.61, 95% confidence interval, 0.51-0.71, p=0.033) for varices at high risk of bleeding. Conclusions: spleen stiffness measurement by transient elastography (FibroScan and ARFI) presented a moderate accuracy and a high positive predictive value to diagnose the presence of esophageal varices. Spleen stifness by FibroScan when associated with platelet/spleen diameter ratio, there is a moderate accuracy with a high specificity to predict varices at high risk of bleeding. However, overlapping values between patients with or without varices was high and this precludes the clinical applicability of these methods Read more Baço Diagnosis Diagnóstico Elasticity imaging techniques Endoscopia Endoscopy Esophageal and gastric varices Hipertensão portal Hypertension portal Spleen Técnicas de imagem por elasticidade Varizes esofágicas e gástricas
150	Turnover do carbono (δ13C) em tecidos corporais e desempenho de leitões desmamados alimentados com dietas contendo nucleotídeos Miassi, Gabriela de Mello. January 2016 (has links) Orientador: Dirlei Antonio Berto / Resumo: Objetivou-se com este estudo avaliar a influência dos nucleotídeos (inosinato e guanilato dissódico) sobre o desempenho, peso relativo e turnover do 13C no intestino delgado, baço, fígado e pâncreas de leitões desmamados com idade média de 21 dias. Foram avaliados os seguintes tratamentos: dieta controle sem suplementação de nucleotídeos (Nu); dietas contendo 0,2% de Nu; 0,4% de Nu e 0,6% de Nu. No primeiro experimento 84 leitões desmamados (6,04 ± 0,25 kg) foram distribuídos em um delineamento experimental em blocos ao acaso com quatro tratamentos (níveis de Nu), sete repetições e três animais por unidade experimental, para avaliação do desempenho. No segundo experimento foram utilizados 87 leitões desmamados (6,03 ± 0,23 kg) em delineamento experimental em blocos ao acaso, com os mesmos tratamentos, sendo abatidos três leitões no dia do desmame (dia zero) e três leitões por tratamento nos dias 3, 5, 8, 12, 23, 35 e 49 após o desmame, para avaliar o turnover do 13C na mucosa e na parede intestinal (duodeno e jejuno), no baço, fígado e pâncreas, e o peso relativo do intestino delgado e do baço, fígado e pâncreas. No primeiro experimento não foi verificado efeito dos tratamentos (P > 0,05) nas variáveis de desempenho dos leitões no período de 21 a 36 dias de idade. No período de 21 a 48 dias de idade dos leitões houve efeito quadrático (P < 0,01) dos níveis de Nu no consumo diário de ração e ganho diário de peso. No período experimental total (21 a 55 dias de idade dos leitões... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: This study was conducted to evaluate effects of dietary supplementation of nucleotide (disodium 5´guanylate and disodium 5´inosinate) on the growth performance, relative weight and carbon turnover 13C of the small intestine, spleen, liver and pancreas of weaned piglets of 21 days of age. The treatments were dietary supplementation with 0% (control); 0.2%; 0.4% or 0.6% nucleotide of diet. In the first trial eighty-four weaned piglets (6.04 ± 0.25 kg average initial BW) were allotted to four dietary treatments (Nu levels) with seven pens per treatment and three pigs per pen, in a randomized complete block design to evaluate the performance. In the second trial eighty-seven weaned piglets (6.03 ± 0.23 kg average initial BW) were used in a randomized complete block design, with the same treatments, and on the day of weaning (day zero) were slaughtered three piglets and days 3, 5, 8, 12, 23, 35 and 49 after weaning, three pigs per treatment were slaughtered, to evaluate the effect of nucleotide on the turnover 13C in the mucosa and intestinal wall (duodenum and jejunum), spleen, liver and pancreas and relative weight of the small intestine and spleen, liver and pancreas. During the first period (21 to 36 days of age), no differences were detected on the performance. During the second period (21 to 48 days of age), a quadratic effect (P < 0.01) of the levels of nucleotide was verified on average daily feed intake and average daily weight gain. During the whole experimental period ... (Complete abstract click electronic access below) / Doutor Read more Aditivos Aditivos. Isótopos estáveis. Suínos. Inosinato dissódico Guanilato dissódico Baço. Figado. Pâncreas. Stable isotopes Disodium 5´guanylate Disodium 5´inosinate Turnover Additives Piglets Liver Spleen Pâncreas.

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