Global ETD Search

31	Sistema automatizado para estimulação elétrica e avaliação da dinâmica do cálcio intracelular em cardiomiócitos derivados de células-tronco pluripotentes induzidas. / Automated system for electrical stimulation and evaluation of intracellular calcium dynamics in induced pluripotent stem cells-derived cardiomyocytes. Veronez, Douglas Martins 15 May 2018 (has links) Este estudo apresenta o desenvolvimento e validação de uma nova abordagem para a avaliação do cálcio intracelular em culturas de cardiomiócitos derivados de células-tronco pluripotentes induzidas humanas (hiPSC-CM - do inglês human induced pluripotent stem cell-derived cardiomyocytes) que pode ser aplicada para avaliar o efeito de drogas no acoplamento excitação-contração. O método consiste na estimulação elétrica e medição conjunta da fluorescência de forma automatizada e foi viabilizado a partir da inclusão de um sistema de estimulação elétrica em um leitor de ELISA (do inglês Enzyme-Linked Immunosorbent Assay). Um estimulador eletrônico compacto foi projetado para operar junto a um leitor de placas gerando pulsos quadrados monofásicos com duração de 5 ms e campo elétrico de 8 Vcm-1 aplicados por microeletrodos metálicos de platina-irídio em células em cultura. Uma placa de cultura normalmente utilizada em leitor de placas foi modificada para permitir a colocação do estimulador e dos eletrodos. A intensidade de fluorescência do cálcio intracelular foi avaliada utilizando um leitor de ELISA durante a estimulação elétrica em culturas de células marcadas com o indicador de Ca2+ Fluo-4 AM. A estimulação elétrica das células resultou em contrações regulares nas frequências de 0,1 Hz; 0,2 Hz; 0,3 Hz e 0,5 Hz induzidas pelo estimulador. Parâmetros dos transientes de cálcio foram estudados após a exposição de culturas de células ao Verapamil (0,05; 0,5 e 5,0 µM), a amplitude e a inclinação máxima da fase de subida foram progressivamente reduzidas com doses crescentes da droga. Os dados obtidos demonstraram que o método apresentado permite a avaliação automatizada de transientes de cálcio durante a estimulação elétrica de culturas de hiPSC-CM utilizando o sistema de estimulação em um leitor de ELISA. Esses resultados validaram a aplicabilidade do sistema ao estudo das alterações da dinâmica do cálcio intracelular induzidas por drogas em células sob estimulação elétrica. O sistema de avaliação automatizada desenvolvido pode ser ampliado para realizar a triagem de alto rendimento em bibliotecas de compostos que tem como alvo o acoplamento excitação-contração em células cardíacas humanas in vitro. / This study presents the development and validation of a new approach for the evaluation of intracellular calcium in cultures of cardiomyocytes derived from human induced pluripotent stem cells (hiPSC-CM), which can be applied to evaluate the effect of drugs on excitation-contraction coupling. The method consists of electrical stimulation and joint measurement of fluorescence in an automated manner and was made possible by the inclusion of an electrical stimulation system in an ELISA (Enzyme-Linked Immunosorbent Assay). A compact electronic stimulator was designed to operate inside a plate reader generating monophasic square pulses with duration of 5 ms and electric field of 8 Vcm-1 applied by platinum-iridium metal microelectrodes to cells in culture. A culture plate used in a plate reader was modified to allow placement of the stimulator and electrodes. Fluorescence intensity of intracellular calcium was measured during electrical stimulation of cell cultures loaded with Ca2+ Fluo-4 AM indicator using a plate reader. The electrical stimulation of the cells generated regularly spaced contractions following the pace of the stimulator at the frequencies of 0.1 Hz, 0.2 Hz, 0.3 Hz and 0.5 Hz. Transient profile parameters were studied after treating cell cultures with Verapamil (0.05, 0.5 and 5.0 µM) the amplitude and the maximum slope of rising phase were progressively reduced with increasing verapamil doses. The data obtained demonstrated that the method presented allows the automated evaluation of calcium transients during the electrical stimulation of hiPSC-CM cultures using the stimulation system in an ELISA reader. These results demonstrated the applicability of the system to the study of changes in the intracellular calcium dynamics induced by drugs in electrically stimulated cells. The system developed is amenable to scaling thus allowing high content automated drug library screening for compounds that target the excitationcontraction coupling in human heart cells in vitro. Bioengenharia Bioengineering Cálcio Electrical stimulator for cell cultures Estimulação elétrica Fluorescence measurements Fluorescência Intracellular calcium Miocárdio Plate reader
32	Zur Modulation volumenaktivierter Chloridströme in Endothelzellen Heinke, Stephan 18 August 1998 (has links) Volumeninduzierte Chloridströme wurden bereits in einer Reihe von Zelltypen charakterisiert. In dieser Arbeit wurde die Modulation volumenaktivierte Chloridströme ICl,Vol und der Signalweg zu ihrer Aktivierung untersucht. In Endothelzellen aus der Pulmonalarterie des Rindes (CPAE) wurden der Membranstrom unter Anwendung der 'patch clamp' - Technik und simultan dazu die Konzentration des freien intrazellulären Kalziums [Ca2+]i gemessen. Bisher wurde davon ausgegangen, daß die Aktivierung von ICl,Vol kalziumunabhängig erfolgt. In dieser Arbeit wurde ICl,Vol unter Pufferung des [Ca2+]i mit BAPTA und EGTA gemessen. Es konnte gezeigt werden, daß freies intrazelluläres Kalzium in Konzentrationen niedriger als 50 nM zur Stromaktivierung notwendig ist. Bei einer höheren Konzentration verliert der Strom jedoch seine Kalziumabhängigkeit. Chromoglycinsäure (CL) blockiert ICl,Vol in Endothelzellen. Dieser Effekt ist jedoch im Vergleich zu dem klassischen Chloridkanalblocker NPPB geringer (Ki=15mM) und sehr langsam (im Mittel 100 s). Damit sind die blockierenden Eigenschaften auch geringer ausgeprägt als z.B. auf ICl,Vol und Hemmung der Serotoninsekretion in Mastzellen. Weiterhin war die Rolle von durch Proteinphosphorylierung modulierten intrazellulären Signalwegen bei der Aktivierung von ICl,Vol Gegenstand von Experimenten. Weder die Aktivierung der Proteinkinase C (PKC) durch direkte Applikation des Phorbolesters PMA noch deren Ab - Regulation durch 24-stündige Inkubation mit PMA hatten Einfluß auf die Aktivierung von ICl,Vol. Auch Wortmannin, ein Inhibitor sowohl der MAP - Kinasen (und damit des Tyrosinkinase - assoziierten Rezeptor - Signalweges) als auch der PI3 - Kinase, zeigte keinen Effekt auf ICl,Vol. Der Aktivator der MAP - Kinasen und der fokalen Adhaesionskinase p125FAK, die Substanz Lysophosphatsäure (LPA), zeigte weder einen Effekt auf ICl,Vol, noch konnte damit ein Chloridstrom induziert werden. Die Induktion von HSP durch Applizierung von thermischem und chemischem Streß unter Inkubation bei bis zu 45 °C über 60 min und Einwirkung von 0,3 mM Natriumarsenit zeigte keinerlei Einfluß auf ICl,Vol. Es konnte auch keine Aktivierung eines Chloridstromes beobachtet werden. Zur Untersuchung des Aktivierungsmechanismus von ICl,Vol dienten Experimente unter gleichzeitiger Messung von ICl,Vol, Membrankapazität (CM) und (jedoch zeitlich unabhängig voneinander) der Zellhöhe. Die Ergebnisse wurden an Hand dreier Modellvorstellungen zur Aktivierung von ICl,Vol diskutiert. Es bestand eine enge Korrelation zwischen Veränderungen der Zellhöhe und des aktivierten Stromes. Beide korrelieren jedoch nicht mit den Änderungen von CM. Dabei änderte sich CM bei einem Teil der Zellen praktisch nicht, d.h. geringer als 2% des Ausgangswertes vor Applikation hypotoner Lösung (n=17), bei den verbliebenen Teil zeigten sich deutliche Veränderungen von durchschnittlich 10,6 ± 0,9 % ( ± SEM, n=5). In letzterem Fall änderte sich jedoch immer zuerst ICl,Vol und dann CM. Nach Inhibierung des intrazellulären Vesikeltransports durch Brefeldin A war ICl,Vol ohne signifikante Änderungen auslösbar. Unter Cycloheximid, einem Blocker der Proteinsynthese auf Transkribtionssebene, wurden keine spezifischen Veränderungen von ICl,Vol beobachtet. Auf jeden Fall ist CM nicht der primäre Trigger für ICl,Vol. Die Aktivierung von volumeninduzierten Chloridströmen erfolgt nicht maßgeblich durch die Inkorporierung von Ionenkanal - Proteinen enthaltenden Membranvesikeln. / Volume-induced chlorid currents are characterised for many types of cells. I have investigated the modulation and activation of these currents. In cultered pulmonary artery endothelial cells (CPAE) patch clamp maesurements of membrane currents and simultaneous maesurements of free intracellular calcium ([Ca2+]i) were performed. Until now, activation of ICl,Vol was characterised as Calcium-independently. I maesured the current buffering [Ca2+]i with the Calcium chelators BAPTA and EGTA. It could be observed, that [Ca2+]i at concentrations less than 50 nM is required to activate ICl,Vol. At higher concentrations, there is no modulation by [Ca2+]i. Sodiumchromoglycate (CL) blocks ICl,Vol in endothelium cells. This effect is small (Ki=15mM) and slow (100 s) as compared of those of the classical chlorid channel blocker NPPB. Inhibitory effects of CL to ICl,Vol in endothelial cells are weaker than to ICl,Vol and to secretion of serotonin in mast cells. The role of intracellular phosphorylation signal pathways on activation of ICl,Vol was investigated. Neither activation of protein kinase C (PKC) throught direct application of the phorbol ester PMA nor down-regulation through preincubation with PMA had any effect on activation of ICl,Vol. Also Wortmannin, an inhibitor of MAP-kinases, failed to have significant effects on I Chlorid-Kanäle Endothel patch clamp intrazelluläres Kalzium chlorid currents endothelium patch clamp intracellular calcium 610 Medizin 33 Medizin WE 5400 WE 5460 ddc:610
33	Sistema automatizado para estimulação elétrica e avaliação da dinâmica do cálcio intracelular em cardiomiócitos derivados de células-tronco pluripotentes induzidas. / Automated system for electrical stimulation and evaluation of intracellular calcium dynamics in induced pluripotent stem cells-derived cardiomyocytes. Douglas Martins Veronez 15 May 2018 (has links) Este estudo apresenta o desenvolvimento e validação de uma nova abordagem para a avaliação do cálcio intracelular em culturas de cardiomiócitos derivados de células-tronco pluripotentes induzidas humanas (hiPSC-CM - do inglês human induced pluripotent stem cell-derived cardiomyocytes) que pode ser aplicada para avaliar o efeito de drogas no acoplamento excitação-contração. O método consiste na estimulação elétrica e medição conjunta da fluorescência de forma automatizada e foi viabilizado a partir da inclusão de um sistema de estimulação elétrica em um leitor de ELISA (do inglês Enzyme-Linked Immunosorbent Assay). Um estimulador eletrônico compacto foi projetado para operar junto a um leitor de placas gerando pulsos quadrados monofásicos com duração de 5 ms e campo elétrico de 8 Vcm-1 aplicados por microeletrodos metálicos de platina-irídio em células em cultura. Uma placa de cultura normalmente utilizada em leitor de placas foi modificada para permitir a colocação do estimulador e dos eletrodos. A intensidade de fluorescência do cálcio intracelular foi avaliada utilizando um leitor de ELISA durante a estimulação elétrica em culturas de células marcadas com o indicador de Ca2+ Fluo-4 AM. A estimulação elétrica das células resultou em contrações regulares nas frequências de 0,1 Hz; 0,2 Hz; 0,3 Hz e 0,5 Hz induzidas pelo estimulador. Parâmetros dos transientes de cálcio foram estudados após a exposição de culturas de células ao Verapamil (0,05; 0,5 e 5,0 µM), a amplitude e a inclinação máxima da fase de subida foram progressivamente reduzidas com doses crescentes da droga. Os dados obtidos demonstraram que o método apresentado permite a avaliação automatizada de transientes de cálcio durante a estimulação elétrica de culturas de hiPSC-CM utilizando o sistema de estimulação em um leitor de ELISA. Esses resultados validaram a aplicabilidade do sistema ao estudo das alterações da dinâmica do cálcio intracelular induzidas por drogas em células sob estimulação elétrica. O sistema de avaliação automatizada desenvolvido pode ser ampliado para realizar a triagem de alto rendimento em bibliotecas de compostos que tem como alvo o acoplamento excitação-contração em células cardíacas humanas in vitro. / This study presents the development and validation of a new approach for the evaluation of intracellular calcium in cultures of cardiomyocytes derived from human induced pluripotent stem cells (hiPSC-CM), which can be applied to evaluate the effect of drugs on excitation-contraction coupling. The method consists of electrical stimulation and joint measurement of fluorescence in an automated manner and was made possible by the inclusion of an electrical stimulation system in an ELISA (Enzyme-Linked Immunosorbent Assay). A compact electronic stimulator was designed to operate inside a plate reader generating monophasic square pulses with duration of 5 ms and electric field of 8 Vcm-1 applied by platinum-iridium metal microelectrodes to cells in culture. A culture plate used in a plate reader was modified to allow placement of the stimulator and electrodes. Fluorescence intensity of intracellular calcium was measured during electrical stimulation of cell cultures loaded with Ca2+ Fluo-4 AM indicator using a plate reader. The electrical stimulation of the cells generated regularly spaced contractions following the pace of the stimulator at the frequencies of 0.1 Hz, 0.2 Hz, 0.3 Hz and 0.5 Hz. Transient profile parameters were studied after treating cell cultures with Verapamil (0.05, 0.5 and 5.0 µM) the amplitude and the maximum slope of rising phase were progressively reduced with increasing verapamil doses. The data obtained demonstrated that the method presented allows the automated evaluation of calcium transients during the electrical stimulation of hiPSC-CM cultures using the stimulation system in an ELISA reader. These results demonstrated the applicability of the system to the study of changes in the intracellular calcium dynamics induced by drugs in electrically stimulated cells. The system developed is amenable to scaling thus allowing high content automated drug library screening for compounds that target the excitationcontraction coupling in human heart cells in vitro. Bioengenharia Cálcio Estimulação elétrica Fluorescência Miocárdio Bioengineering Electrical stimulator for cell cultures Fluorescence measurements Intracellular calcium Plate reader
34	Caractérisation et implication du canal cationique TRPV1 dans la physiopathologie du muscle strié squelettique / Characterisation and implication of TRPV1 cationic channel in physiopathology of skeletal muscle Lotteau, Sabine 10 October 2013 (has links) Le canal cationique TRPV1 (Transient Receptor Potential Vanilloid 1) est activé par la capsaïcine, une acidose, de fortes températures ainsi que par les anesthésiques volatils (AV) dans les neurones sensoriels. Dans le muscle squelettique, TRPV1 est impliqué dans le métabolisme énergétique et l'exercice d'endurance. Grâce à des techniques d'immunomarquage et d'imagerie calcique, la première partie de la thèse vise à caractériser TRPV1 en tant que canal de fuite fonctionnel du réticulum sarcoplasmique (RS) dans les cellules musculaires squelettiques isolées de FDB (Flexor Digitorum Brevis) de souris. Par la suite, nous nous sommes intéressés à son rôle physiopathologique dans le muscle strié squelettique. Ainsi, dans une seconde partie nous supposons une implication de TRPV1 dans les crises d'hyperthermie maligne (HM) chez l'homme. Cette pathologie musculaire correspond à une crise de métabolisme exacerbé du muscle strié squelettique menant à une brusque montée en température chez le patient (>42°C) endormi au moyen d'AV. Dans cette deuxième étude nous démontrons, à travers une approche combinant imagerie calcique et outils pharmacologiques spécifiques du canal, que TRPV1 est activé lors de l'exposition des cellules musculaires à l'isoflurane. TRPV1 est donc une cible des AV dans la cellule musculaire. Puis, des variants de TRPV1 (T612M et N394del) de patients susceptibles à l'HM ont été découvertes. Nous avons pu montrer, suite à la transfection in vivo de ces variants dans des souris déficientes en TRPV1 et grâce à la mesure de flux calciques intracellulaires, que les variants humains de TRPV1 rendent ces canaux plus sensibles aux anesthésiques volatils que le canal TRPV1 humain sauvage. La troisième partie de la thèse a pour but de déterminer le rôle de TRPV1 dans le muscle squelettique en conditions physiologiques par des études fonctionnelles (fonction locomotrice, consommation d'oxygène) sur animal entier. Les résultats préliminaires de cette étude tendent à montrer que l'entraînement physique est moins efficace sur la fonction musculaire des souris déficientes en TRPV1. En conclusion, l'ensemble de ces résultats révèlent pour la première fois que TRPV1 est un canal calcique de fuite fonctionnel du RS pouvant faire le lien entre le déclenchement de l'HM au cours des anesthésies et la présence des RyR1 mutés dans le muscle squelettique / TRPV1 (Transient Receptor Potential Vanilloid 1) cation channel is activated by capsaicine, acidosis, high temperature and by volatile anaesthetics (VA) in sensory neurons. In skeletal muscle, TRPV1 appears to be implied in exercice endurance and energy metabolism. The present work aims first to characterize the functionality of this channel using immnostaining and calcium imaging. We report that TRPV1 is functionally expressed in isolated mouse skeletal muscle cells of FDB (Flexor Digitorum Brevis). These experiments point out that TRPV1 acts as a SR calcium leak channel. In contrast to earlier reports, our analysis shows that TRPV1 is only located to the sarcoplasmic reticulum (SR) membrane. Subsequently, we have studied its physiological role in skeletal muscle. Thus, in a second part, we suppose that TRPV1 could be involved in malignant hyperthermia (MH) crisis in human. MH is a muscular pathology linked to an abrupt increase in body temperature (> 42°C) in patients. MH crisis is a severe and feared complication of anesthesia. Nevertheless, any studies have demonstrated that RyR1 mutants are activated by VA. If the triggering agents of MH are known, their targets remain to be determined. By combining calcium imaging and pharmacological agents, our data first demonstrate that TRPV1 is activated by isoflurane in skeletal muscle cells. TRPV1 is so a target of volatile anaesthetics in skeletal muscle. Afterwards, TRPV1 mutants (T612M and N394del), obtained from susceptibles MH patients, were discovered. In the second part of the work, using in vivo transfection of TRPV1 mutants in TRPV1-/- mice and intracellular calcium measurements we have been able to demonstrate that human TRPV1 mutants are more sensitive to VA than human wild type TRPV1. The last part of the work investigates the physiological role of TRPV1 in skeletal muscle, using a functional exploration (locomotor function, oxygen consumption) in TRPV1-/- mice. Preliminary data point out that training seems to be less effective on skeletal muscle function of TRPV1-/- mice. To conclude, these results indicate for the first time that TRPV1 is a functional SR calcium leak channel and that TRPV1 may be the missing link between MH induction and RyR1 mutants in skeletal muscle during anesthesia Canaux calciques Muscle squelettique Canaux TRPV1 Hyperthermie maligne Calcium intracellulaire Calcium channels Skeletal muscle TRPV1 channel Malignant hyperthermia Intracellular calcium 573.75
35	The Duodenal Mucosal Bicarbonate Secretion : Role of Melatonin in Neurohumoral Control and Cellular Signaling Sjöblom, Markus January 2003 (has links) <p>The duodenal lumen is exposed to aggressive factors with a high potential to cause damage to the mucosa. Bicarbonate secretion by the duodenal mucosa is accepted as the primary important defense mechanism against the hydrochloric acid intermittently expelled from the stomach.</p><p>The present thesis concerns the influence of the central nervous system and the effects of the hormone melatonin on bicarbonate secretion in anesthetized rats in vivo. Effects of melatonin on intracellular calcium signaling by duodenal enterocyte in vitro were examined in tissues of both human and rat origin. The main findings were as follows:</p><p>Melatonin is a potent stimulant of duodenal mucosal bicarbonate secretion and also seems to be involved in the acid-induced stimulation of the secretion. Stimulation elicited in the central nervous system by the α1-adrenoceptor agonist phenylephrine induced release of melatonin from the intestinal mucosa and a four-fold increase in alkaline secretion. The melatonin antagonist luzindole abolished the duodenal secretory response to administered melatonin and to central nervous phenylephrine but did not influence the release of intestinal melatonin. Central nervous stimulation was also abolished by synchronous ligation of the vagal trunks and the sympathetic chains at the sub-laryngeal level. </p><p>Melatonin induced release of calcium from intracellular stores and also influx of extracellular calcium in isolated duodenal enterocytes. Enterocytes in clusters functioned as a syncytium.</p><p>Overnight fasting rapidly and profoundly down-regulated the responses to the duodenal secretagogues orexin-A and bethanechol but not those to melatonin or vasoactive intestinal polypeptide.</p><p>In conclusion, the results strongly suggest that intestinal melatonin plays an important role in central nervous elicited stimulation of duodenal mucosal bicarbonate secretion. Sensitivity of this alkaline secretion to some peripheral stimulators markedly depends on the feeding status.</p> Physiology alkaline secretion central nervous system duodenal enterocyte duodenal ulcer duodenum enterochromaffin cell human intraarterial intracellular calcium intracerebroventricular melatonin rat vagal nerve Fysiologi Physiology Fysiologi
36	The Duodenal Mucosal Bicarbonate Secretion : Role of Melatonin in Neurohumoral Control and Cellular Signaling Sjöblom, Markus January 2003 (has links) The duodenal lumen is exposed to aggressive factors with a high potential to cause damage to the mucosa. Bicarbonate secretion by the duodenal mucosa is accepted as the primary important defense mechanism against the hydrochloric acid intermittently expelled from the stomach. The present thesis concerns the influence of the central nervous system and the effects of the hormone melatonin on bicarbonate secretion in anesthetized rats in vivo. Effects of melatonin on intracellular calcium signaling by duodenal enterocyte in vitro were examined in tissues of both human and rat origin. The main findings were as follows: Melatonin is a potent stimulant of duodenal mucosal bicarbonate secretion and also seems to be involved in the acid-induced stimulation of the secretion. Stimulation elicited in the central nervous system by the α1-adrenoceptor agonist phenylephrine induced release of melatonin from the intestinal mucosa and a four-fold increase in alkaline secretion. The melatonin antagonist luzindole abolished the duodenal secretory response to administered melatonin and to central nervous phenylephrine but did not influence the release of intestinal melatonin. Central nervous stimulation was also abolished by synchronous ligation of the vagal trunks and the sympathetic chains at the sub-laryngeal level. Melatonin induced release of calcium from intracellular stores and also influx of extracellular calcium in isolated duodenal enterocytes. Enterocytes in clusters functioned as a syncytium. Overnight fasting rapidly and profoundly down-regulated the responses to the duodenal secretagogues orexin-A and bethanechol but not those to melatonin or vasoactive intestinal polypeptide. In conclusion, the results strongly suggest that intestinal melatonin plays an important role in central nervous elicited stimulation of duodenal mucosal bicarbonate secretion. Sensitivity of this alkaline secretion to some peripheral stimulators markedly depends on the feeding status. Physiology alkaline secretion central nervous system duodenal enterocyte duodenal ulcer duodenum enterochromaffin cell human intraarterial intracellular calcium intracerebroventricular melatonin rat vagal nerve Fysiologi Physiology Fysiologi
37	Alterations in lymphocyte signalling produced by exposure to mercury Yole, Margaret Jane 03 July 2007 The effects of 1 min 4 hr exposures to mercuric chloride (HgCl2), methyl mercuric chloride (CH3HgCl), p-chloromercuribenzoate (p-CMB) and ethylmercurithiosalicylate (TMS) on cell viability and kinetics of cell death, microtubules, F-actin, CD3 receptor expression, protein tyrosine phosphorylation (PTyr-P), intracellular calcium [Ca2+]i and responses to polarized signals in YAC-1 lymphoma cells were investigated. We hypothesized that immunotoxic effects of HgCl2 (Hg2+) are initiated by global receptor triggering, accompanied by increased protein tyrosine phosphorylation (PTyr-P) and down-regulation of the T-cell receptor (TCR). As a polychloride anion with poor lipid solubility, inorganic Hg2+ may produce effects at the outer cell membrane before significant intracellular accumulation, loss of microtubule integrity (a sensitive target) and activation of cell death through apoptotic pathways. The organomercurial compound p-CMB is likewise thought to penetrate membranes slowly as a result of ionization. In contrast, the highly lipid-soluble organomercurial compounds CH3HgCl and TMS were expected to reduce responses to polarized stimuli only in conjunction with and not prior to loss of microtubule integrity and the onset of necrotic cell death. <p>Two general patterns of effects were observed. In HgCl2-treated YAC-1 cells, inhibition of responses to polarized stimuli preceded loss of microtubules and onset of cell death. Effects on polarized stimuli were preceded by a transient Ca2+ signal; however, this Ca2+ signal appeared abortive, accompanied by a paradoxic decrease in PTyr-P and partial down-regulation of CD3 receptors. Responses to polarised stimuli were inhibited prior to extensive loss of microtubule staining, indicating effects preceded cytosolic Hg2+ accumulation. HgCl2 exposure was followed rapidly by necrotic cell death. <p>Similarly, p-CMB-treated YAC-1 cells failed to respond to polarized stimuli before effects on microtubules or loss of viability, and proceeded rapidly to late apoptosis; however, a transient Ca2+ signal and progressive loss of F-actin preceded effects in all other assays and may account for loss of polarized responses. <p>In CH3HgCl- and TMS-treated YAC-1 cells, CD3 receptor expression, [Ca2+] and PTyr-P were increased immediately, along with loss of microtubules. These reductions preceded inhibition of polarized signaling responses and seemed to indicate a general loss of cellular homeostasis not seen in HgCl2- and p-CMB-treated cells; loss of homeostasis did not necessarily produce simultaneous loss of viability, as TMS-treated cells remained viable for 30 min while CH3HgCl-treated cells became apoptotic within 1 min. Nonetheless, the YAC-1 cells proceeded to cell death more slowly, remaining early apoptotic after 4 hr, when almost all HgCl2- and p-CMB-treated cells were necrotic. These findings indicate the two groups of mercury compounds may alter responses to polarized stimuli and induce cell death by distinct pathways, one involving an apparently abortive signal and the other mediated by much more profound disruption of cellular homeostasis. Within the larger patterns there are further differences between the effects produced by each Hg compound, likely reflecting the combined influence of pharmacokinetic and dynamic factors governing access to and interactions with different cellular targets leading to cell death. These distinct targets may in turn be reflected in the different immune effects produced by these compounds <i>in vivo</i>. methyl mercuric chloride mercuric chloride phosphotyrosine CD3 receptor intracellular calcium microtubles actin immunological synapse organic mercury inorganic mercury p-chloromercuribenzoate thimerosal YAC-1 lymphoma cytotoxicity apoptosis viability
38	Alterations in lymphocyte signalling produced by exposure to mercury Yole, Margaret Jane 03 July 2007 (has links) The effects of 1 min 4 hr exposures to mercuric chloride (HgCl2), methyl mercuric chloride (CH3HgCl), p-chloromercuribenzoate (p-CMB) and ethylmercurithiosalicylate (TMS) on cell viability and kinetics of cell death, microtubules, F-actin, CD3 receptor expression, protein tyrosine phosphorylation (PTyr-P), intracellular calcium [Ca2+]i and responses to polarized signals in YAC-1 lymphoma cells were investigated. We hypothesized that immunotoxic effects of HgCl2 (Hg2+) are initiated by global receptor triggering, accompanied by increased protein tyrosine phosphorylation (PTyr-P) and down-regulation of the T-cell receptor (TCR). As a polychloride anion with poor lipid solubility, inorganic Hg2+ may produce effects at the outer cell membrane before significant intracellular accumulation, loss of microtubule integrity (a sensitive target) and activation of cell death through apoptotic pathways. The organomercurial compound p-CMB is likewise thought to penetrate membranes slowly as a result of ionization. In contrast, the highly lipid-soluble organomercurial compounds CH3HgCl and TMS were expected to reduce responses to polarized stimuli only in conjunction with and not prior to loss of microtubule integrity and the onset of necrotic cell death. <p>Two general patterns of effects were observed. In HgCl2-treated YAC-1 cells, inhibition of responses to polarized stimuli preceded loss of microtubules and onset of cell death. Effects on polarized stimuli were preceded by a transient Ca2+ signal; however, this Ca2+ signal appeared abortive, accompanied by a paradoxic decrease in PTyr-P and partial down-regulation of CD3 receptors. Responses to polarised stimuli were inhibited prior to extensive loss of microtubule staining, indicating effects preceded cytosolic Hg2+ accumulation. HgCl2 exposure was followed rapidly by necrotic cell death. <p>Similarly, p-CMB-treated YAC-1 cells failed to respond to polarized stimuli before effects on microtubules or loss of viability, and proceeded rapidly to late apoptosis; however, a transient Ca2+ signal and progressive loss of F-actin preceded effects in all other assays and may account for loss of polarized responses. <p>In CH3HgCl- and TMS-treated YAC-1 cells, CD3 receptor expression, [Ca2+] and PTyr-P were increased immediately, along with loss of microtubules. These reductions preceded inhibition of polarized signaling responses and seemed to indicate a general loss of cellular homeostasis not seen in HgCl2- and p-CMB-treated cells; loss of homeostasis did not necessarily produce simultaneous loss of viability, as TMS-treated cells remained viable for 30 min while CH3HgCl-treated cells became apoptotic within 1 min. Nonetheless, the YAC-1 cells proceeded to cell death more slowly, remaining early apoptotic after 4 hr, when almost all HgCl2- and p-CMB-treated cells were necrotic. These findings indicate the two groups of mercury compounds may alter responses to polarized stimuli and induce cell death by distinct pathways, one involving an apparently abortive signal and the other mediated by much more profound disruption of cellular homeostasis. Within the larger patterns there are further differences between the effects produced by each Hg compound, likely reflecting the combined influence of pharmacokinetic and dynamic factors governing access to and interactions with different cellular targets leading to cell death. These distinct targets may in turn be reflected in the different immune effects produced by these compounds <i>in vivo</i>. methyl mercuric chloride mercuric chloride phosphotyrosine CD3 receptor intracellular calcium microtubles actin immunological synapse organic mercury inorganic mercury p-chloromercuribenzoate thimerosal YAC-1 lymphoma cytotoxicity apoptosis viability
39	Avaliação da ingestão habitual de cálcio e sua associação com a concentração intracelular de cálcio, adiposidade corporal, perfil metabólico, biomarcadores inflamatórios, pressão arterial e função endotelial Thaís da Silva Ferreira 19 June 2012 (has links) A associação inversa da ingestão de cálcio dietético com adiposidade corporal e pressão arterial está documentada em estudos epidemiológicos. Achados experimentais sugerem que este fenômeno pode ser mediado por alterações na concentração intracelular de cálcio ([Ca]i). Existem poucos estudos relacionando o cálcio dietético com a [Ca]i. O objetivo do presente estudo foi avaliar a relação da ingestão habitual de cálcio dietético com a [Ca]i, adiposidade corporal, perfil metabólico, biomarcadores inflamatórios, pressão arterial e função endotelial em mulheres. Para tanto, foi desenvolvido estudo transversal, com 76 mulheres na pré-menopausa submetidas à avaliação: dietética (questionário de frequência alimentar validado); da [Ca]i em eritrócitos (espectrometria de absorbância atômica); da gordura corporal (GC) total [índice de massa corporal (IMC) e % GC por bioimpedância elétrica] e central [perímetro da cintura (PC), e razão cintura quadril (RCQ)]; do perfil metabólico (glicose, colesterol e frações, insulina e HOMA-IR); dos biomarcadores inflamatórios [adiponectina e proteína C-reativa (PCR)]; dos biomarcadores da função endotelial [molécula de adesão intracelular-1 (ICAM-1), molécula de adesão celular vascular-1 (VCAM-1) e E-Selectina]; da função endotelial avaliada pelo equipamento Endo-PAT2000; e da pressão arterial. Calcitriol, paratormônio, cálcio sérico e cálcio urinário completaram o metabolismo do cálcio. As participantes foram estratificadas em 2 grupos de acordo com a ingestão habitual de cálcio: Grupo com baixa ingestão de cálcio ou BIC (n=32; ingestão de cálcio <600mg/d) e Grupo com elevada ingestão de cálcio ou AIC (n=44; ingestão de cálcio ≥600mg/d). A média da idade foi semelhante entre os grupos (Grupo BIC: 31,41,4 vs Grupo AIC: 31,41,4anos; p=0,99). Após ajustes para fatores de confundimento (idade, ingestão de energia, bebida alcoólica, proteína, carboidratos e lipídios), o Grupo AIC, em comparação com o BIC, apresentou valores significativamente mais baixos de IMC (25,65,3 vs 26,9 6,0 kg/m; p=0,02), PC (84,413,6 vs 87,815,3cm; p=0,04), % GC (31,15,9 vs 33,35,6 %; p=0,003), pressão arterial diastólica (68,210,8 vs 72,411,2 mm Hg; p=0,04) e pressão arterial média (80,1310,94 vs 83,8611,70 mmHg; p=0,04); e significativamente mais altos de HDL-colesterol (58,612,2 vs 52,912,2 mg/dL; p=0,004) e adiponectina (34572,1 19472,8 vs 31910,319385,1 ng/mL; p=0,05). A [Ca]i e as outras variáveis avaliadas não diferiram entre os grupos, mesmo após ajustes. Neste estudo realizado com mulheres, o maior consumo de cálcio se associou com valores mais baixos de adiposidade corporal total e central, pressão arterial diastólica e média; além de valores mais elevados de HDL-colesterol e adiponectina / The inverse association between dietary calcium intake and body adiposity and blood pressure is established in epidemiological studies. Experimental data suggest that it may be mediated by alterations in intracellular calcium concentration ([Ca]i). There are few studies evaluating the relationship beween dietary calcium and [Ca]i. The objective of the present study was to evaluat the association of dietary calcium with [Ca]I, body adiposity, metabolic profile, inflammatory biomarkers, blood pressure, and endothelial function in women. It was conducted an observational and cross-sectional clinical trial, including 76 women with pre-menopausal status who were submitted to the following evaluations: dietary intake (by a food frequency questionnaire); [Ca]I in erythrocytes (by atomic absorption spectrometry); body adiposity (by body mass index [BMI] and electrical bioimpedance; abdominal adiposity (by waist circumference and waist-to-hip-ratio; metabolic profile (by assessing plasma glucose, total cholesterol and fractions, insulin and HOMA-IR); inflammatory biomarkers (adiponectin and C-reactive protein); endothelial function (by analyzing adhesion molecules and by peripheral artery tonometry [PAT]); and blood pressure. Calcitriol, parathyroid hormone, and serum and urinary calcium completed calcium metabolism. Participants were stratified into two groups according to their mean usual dietary calcium intake: low calcium group (LCG; n=32; dietary calcium intake <600mg/d) and high calcium group (HCG; n=44; dietary calcium intake ≥600mg/d). Após ajustes para fatores de confundimento (idade, ingestão de energia, bebida alcoólica, proteína, carboidratos e lipídios), o Grupo AIC, em comparação com o BIC, apresentou valores significativamente mais baixos de IMC (25,65,3 vs 26,9 6,0 kg/m; p=0,02), PC (84,413,6 vs 87,815,3cm; p=0,04), % GC (31,15,9 vs 33,35,6 %; p=0,003), pressão arterial diastólica (68,210,8 vs 72,411,2 mm Hg; p=0,04) e pressão arterial média (80,1310,94 vs 83,8611,70 mmHg; p=0,04); e significativamente mais altos de HDL-colesterol (58,612,2 vs 52,912,2 mg/dL; p=0,004) e adiponectina (34572,1 19472,8 vs 31910,319385,1 ng/mL; p=0,05). A [Ca]i e as outras variáveis avaliadas não diferiram entre os grupos, mesmo após ajustes. Neste estudo realizado com mulheres, o maior consumo de cálcio se associou com valores mais baixos de adiposidade corporal total e central, pressão arterial diastólica e média; além de valores mais elevados de HDL-colesterol e adiponectina. After controlling for potential confounders (age, dietary energy, protein, carbohydrates and lipids and alcohol intake), HCG, in comparison to LCG, showed significantly lower vlaues of BMI (25.65.3 vs 26.9 6.0 kg/m; p=0.02), waist circumference (84.413.6 vs 87.815.3cm; p=0.04), % body fat (31.15.9 vs 33.35.6 %; p=0.003), diastolic blood pressure (68.210.8 vs 72.411.2 mm Hg; p=0.04) e mean blood pressure (80.1310.94 vs 83.8611.70 mmHg; p=0.04); and significantly higher values of HDL-cholesterol (58.612.2 vs 52.912.2 mg/dl; p=0.004) and adiponectin (34.5719.47 vs 31.9119.39 μg/ml; p=0.05). There was no difference between groups in relation to [Ca]i and other parameters evaluated, even after adjusting for confounding factors. In this study, higher dietary calcium intake was associated with lower values of total and abdominal adiposity, diastolic and mean blood pressure; and with higher values of HDL-cholesterol e adiponectin Cálcio dietético Cálcio intracelular Adiposidade Função endotelial Cálcio no organismo Cálcio - Metabolismo Cálcio na nutrição humana Pressão arterial Dietary calcium Intracellular calcium Adiposity Endothelial function DIETETICA
40	Avaliação da ingestão habitual de cálcio e sua associação com a concentração intracelular de cálcio, adiposidade corporal, perfil metabólico, biomarcadores inflamatórios, pressão arterial e função endotelial Thaís da Silva Ferreira 19 June 2012 (has links) A associação inversa da ingestão de cálcio dietético com adiposidade corporal e pressão arterial está documentada em estudos epidemiológicos. Achados experimentais sugerem que este fenômeno pode ser mediado por alterações na concentração intracelular de cálcio ([Ca]i). Existem poucos estudos relacionando o cálcio dietético com a [Ca]i. O objetivo do presente estudo foi avaliar a relação da ingestão habitual de cálcio dietético com a [Ca]i, adiposidade corporal, perfil metabólico, biomarcadores inflamatórios, pressão arterial e função endotelial em mulheres. Para tanto, foi desenvolvido estudo transversal, com 76 mulheres na pré-menopausa submetidas à avaliação: dietética (questionário de frequência alimentar validado); da [Ca]i em eritrócitos (espectrometria de absorbância atômica); da gordura corporal (GC) total [índice de massa corporal (IMC) e % GC por bioimpedância elétrica] e central [perímetro da cintura (PC), e razão cintura quadril (RCQ)]; do perfil metabólico (glicose, colesterol e frações, insulina e HOMA-IR); dos biomarcadores inflamatórios [adiponectina e proteína C-reativa (PCR)]; dos biomarcadores da função endotelial [molécula de adesão intracelular-1 (ICAM-1), molécula de adesão celular vascular-1 (VCAM-1) e E-Selectina]; da função endotelial avaliada pelo equipamento Endo-PAT2000; e da pressão arterial. Calcitriol, paratormônio, cálcio sérico e cálcio urinário completaram o metabolismo do cálcio. As participantes foram estratificadas em 2 grupos de acordo com a ingestão habitual de cálcio: Grupo com baixa ingestão de cálcio ou BIC (n=32; ingestão de cálcio <600mg/d) e Grupo com elevada ingestão de cálcio ou AIC (n=44; ingestão de cálcio ≥600mg/d). A média da idade foi semelhante entre os grupos (Grupo BIC: 31,41,4 vs Grupo AIC: 31,41,4anos; p=0,99). Após ajustes para fatores de confundimento (idade, ingestão de energia, bebida alcoólica, proteína, carboidratos e lipídios), o Grupo AIC, em comparação com o BIC, apresentou valores significativamente mais baixos de IMC (25,65,3 vs 26,9 6,0 kg/m; p=0,02), PC (84,413,6 vs 87,815,3cm; p=0,04), % GC (31,15,9 vs 33,35,6 %; p=0,003), pressão arterial diastólica (68,210,8 vs 72,411,2 mm Hg; p=0,04) e pressão arterial média (80,1310,94 vs 83,8611,70 mmHg; p=0,04); e significativamente mais altos de HDL-colesterol (58,612,2 vs 52,912,2 mg/dL; p=0,004) e adiponectina (34572,1 19472,8 vs 31910,319385,1 ng/mL; p=0,05). A [Ca]i e as outras variáveis avaliadas não diferiram entre os grupos, mesmo após ajustes. Neste estudo realizado com mulheres, o maior consumo de cálcio se associou com valores mais baixos de adiposidade corporal total e central, pressão arterial diastólica e média; além de valores mais elevados de HDL-colesterol e adiponectina / The inverse association between dietary calcium intake and body adiposity and blood pressure is established in epidemiological studies. Experimental data suggest that it may be mediated by alterations in intracellular calcium concentration ([Ca]i). There are few studies evaluating the relationship beween dietary calcium and [Ca]i. The objective of the present study was to evaluat the association of dietary calcium with [Ca]I, body adiposity, metabolic profile, inflammatory biomarkers, blood pressure, and endothelial function in women. It was conducted an observational and cross-sectional clinical trial, including 76 women with pre-menopausal status who were submitted to the following evaluations: dietary intake (by a food frequency questionnaire); [Ca]I in erythrocytes (by atomic absorption spectrometry); body adiposity (by body mass index [BMI] and electrical bioimpedance; abdominal adiposity (by waist circumference and waist-to-hip-ratio; metabolic profile (by assessing plasma glucose, total cholesterol and fractions, insulin and HOMA-IR); inflammatory biomarkers (adiponectin and C-reactive protein); endothelial function (by analyzing adhesion molecules and by peripheral artery tonometry [PAT]); and blood pressure. Calcitriol, parathyroid hormone, and serum and urinary calcium completed calcium metabolism. Participants were stratified into two groups according to their mean usual dietary calcium intake: low calcium group (LCG; n=32; dietary calcium intake <600mg/d) and high calcium group (HCG; n=44; dietary calcium intake ≥600mg/d). Após ajustes para fatores de confundimento (idade, ingestão de energia, bebida alcoólica, proteína, carboidratos e lipídios), o Grupo AIC, em comparação com o BIC, apresentou valores significativamente mais baixos de IMC (25,65,3 vs 26,9 6,0 kg/m; p=0,02), PC (84,413,6 vs 87,815,3cm; p=0,04), % GC (31,15,9 vs 33,35,6 %; p=0,003), pressão arterial diastólica (68,210,8 vs 72,411,2 mm Hg; p=0,04) e pressão arterial média (80,1310,94 vs 83,8611,70 mmHg; p=0,04); e significativamente mais altos de HDL-colesterol (58,612,2 vs 52,912,2 mg/dL; p=0,004) e adiponectina (34572,1 19472,8 vs 31910,319385,1 ng/mL; p=0,05). A [Ca]i e as outras variáveis avaliadas não diferiram entre os grupos, mesmo após ajustes. Neste estudo realizado com mulheres, o maior consumo de cálcio se associou com valores mais baixos de adiposidade corporal total e central, pressão arterial diastólica e média; além de valores mais elevados de HDL-colesterol e adiponectina. After controlling for potential confounders (age, dietary energy, protein, carbohydrates and lipids and alcohol intake), HCG, in comparison to LCG, showed significantly lower vlaues of BMI (25.65.3 vs 26.9 6.0 kg/m; p=0.02), waist circumference (84.413.6 vs 87.815.3cm; p=0.04), % body fat (31.15.9 vs 33.35.6 %; p=0.003), diastolic blood pressure (68.210.8 vs 72.411.2 mm Hg; p=0.04) e mean blood pressure (80.1310.94 vs 83.8611.70 mmHg; p=0.04); and significantly higher values of HDL-cholesterol (58.612.2 vs 52.912.2 mg/dl; p=0.004) and adiponectin (34.5719.47 vs 31.9119.39 μg/ml; p=0.05). There was no difference between groups in relation to [Ca]i and other parameters evaluated, even after adjusting for confounding factors. In this study, higher dietary calcium intake was associated with lower values of total and abdominal adiposity, diastolic and mean blood pressure; and with higher values of HDL-cholesterol e adiponectin Cálcio dietético Cálcio intracelular Adiposidade Função endotelial Cálcio no organismo Cálcio - Metabolismo Cálcio na nutrição humana Pressão arterial Dietary calcium Intracellular calcium Adiposity Endothelial function DIETETICA

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