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Characterization of the Second Messenger Signaling Cascade Linking Angiotensin II Receptor Activation with Vascular Smooth Muscle Cell MitogenesisWildroudt, Maria L. 28 July 2005 (has links)
No description available.
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Arachidonic acid-containing phosphatidylcholine species are increased in selected brain regions of a depressive animal model: implications for pathophysiology.Green, P., Anyakoha, Ngozi G., Gispan-Herman, I,, Yadid, G., Nicolaou, Anna January 2009 (has links)
No / The Flinders Sensitive Line (FSL) rat is a genetic animal model of depression. Following recent findings that the brain fatty acid composition of FSL is characterised by increased arachidonic acid (AA), we used electrospray tandem mass spectrometry and 1H-NMR to examine lipid species in different brain areas. Cholesterol and sphingolipids were increased in the hypothalamus of the FSL rats. Furthermore, arachidonic acid-containing phosphatidylcholine species (AA-PC) were elevated with PC16:0/20:4, PC18:1/20:4 and PC18:0/20:4 (p<0.003) increased in the hypothalamus and striatum. In contrast, there was a decrease in some docosahexaenoic acid (DHA)-containing species, specifically PC18:1/22:6 (p<0.003) in the striatum and PE18:1/22:6 (p<0.004) in the prefrontal cortex. Since no significant differences were observed in the erythrocyte fatty acid concentrations, dietary or environmental causes for these observations are unlikely. The increase in AA-PC species which in this animal model may be associated with altered neuropathy target esterase activity, an enzyme involved in membrane PC homeostasis, may contribute to the depressive phenotype of the FSL rats.
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The CHSE-214 salmon cell line as a model to study molecular regulation of long-chain polyunsaturated fatty acid biosynthesis in salmonidsRubio Mejia, Olga Liliana January 2015 (has links)
The main source of omega-3 (n-3) long-chain polyunsaturated fatty acids (LC-PUFA) in our diet is supplied by fish, and an ever-increasing proportion of these are being produced by aquaculture. The drive for the growing market demand and production from sustainable sources has led to the use of high-energy (fat) diets and, recently, to the replacement of fishmeal and fish oil with non-marine components, such as plant meals and vegetable oils that are devoid of n-3 LC-PUFA. Both changes impact greatly on lipid and fatty acid metabolism in fish, with health implications for the fish and the human consumer. This impact highlights the need to investigate the basic molecular mechanisms underlying the regulation of lipid and fatty acid metabolism in fish, specifically focussing on the pathways of lipid homeostasis and LC-PUFA synthesis. The aim of this study was to develop and utilise Chinook salmon embryo (CHSE-214) cell line as a model for Atlantic salmon, Salmo salar L., to enable an integrated approach to study the biochemical and molecular regulation of lipid metabolism in fish. In particular, α-linolenic acid (LNA, 18:3n-3) and linoleic acid (LOA, 18:2n-6), which are essential fatty acids abundantly found in vegetable oils, and are precursors of LC-PUFA, were supplemented in combination with other fatty acids, to explore the effect of these on total lipid content, lipid class, FA composition and gene expression of CHSE-214 cell line. Total lipid content was extracted, followed by determination of lipid class and fatty acid analyses. Gene expression analyses of transcription/nuclear factors and various target genes in Atlantic salmon, including those involved in pathways of LC-PUFA synthesis and fatty acid oxidation, were carried out. The results demonstrated that CHSE-214 cell line, under experimental conditions, is able to convert LNA to eicosapentaenoic acid (EPA, 20:5n-3), and LOA to arachidonic acid (ARA, 20:4n-6), but not LNA and/or EPA to docosahexaenoic acid (DHA, 22:6n-3), highlighting the activity of elongase and desaturase enzymes during the conversion process. Changes occurring on the fatty acid profile and also at molecular level were observed. Understanding the role that transcription factors play in the regulation of lipid biosynthesis in fish will allow endogenous LC-PUFA synthesis to be optimised. The results from this study could be used to improve the efficiency of alternative, sustainable diets in aquaculture, while maintaining the nutritional quality of farmed fish for the final consumer. CHSE-214 cell line can therefore be used as a model to study the molecular mechanisms involved in the LC-PUFA biosynthesis, particularly in the conversion of LNA to EPA, which can then be reproduced in vivo, saving time and money.
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Caractérisation de nouvelles cibles de LXR et impact sur le métabolisme lipidique et l'athérosclérose / Characterization of new LXR target genes and consequences on lipid metabolism and atherosclerosisVarin, Alexis 21 October 2014 (has links)
Les récepteurs nucléaires LXRα et LXRβ sont activés par la fixation de dérivés oxygénés du cholestérol. Ils régulent l’expression de nombreux gènes appartenant au métabolisme du cholestérol et des acides gras, et jouent un rôle important dans l’inflammation et l’immunité innée. L’activation de LXR inhibe le développement de l’athérosclérose, en augmentant l’efflux de cholestérol des macrophages ainsi que le transport inverse jusqu’au foie et l’excrétion biliaire. De plus, LXR diminue la biosynthèse et la captation du cholestérol dans les tissus périphériques. Enfin, les agonistes synthétiques de LXR administrés à des souris diminuent significativement l’inflammation dans les lésions athérosclérotiques, notamment en inhibant la sécrétion de certaines cytokines inflammatoires. Néanmoins LXR régule également la lipogenèse et la synthèse d’acides gras mono-insaturés, et l’administration d’agonistes de LXR s’accompagne également d’effets indésirables liés à cette régulation, comme une accumulation dérégulée d’acides gras dans le foie et une augmentation du taux de LDLs circulantes. Plusieurs autres mécanismes restent encore à être explorés, comme la synthèse d’acides gras polyinsaturés et les conséquences sur le métabolisme cellulaire. Nos travaux identifient une nouvelle voie régulée entièrement par LXR, le métabolisme des acides gras polyinsaturés. Le récepteur nucléaire LXR régule l’ensemble des enzymes FADS1, FADS2 et ELOVL5, responsables de la synthèse d’acides gras polyinsaturés oméga-6 et oméga-3. Cette régulation s’accompagne d’une incorporation d’acide arachidonique dans les phospholipides, via la régulation de LPCAT3, ce qui prépare les macrophages à une synthèse accrue de dérivés inflammatoires issus de l’acide arachidonique, comme la Prostaglandine E2, suite à une stimulation au lipopolysaccharide. La régulation de cette voie par LXR a également un effet sur le développement de l’athérosclérose, augmentant les taux d’acides gras polyinsaturés oméga-6 et oméga-3 dans les plaques d’athérome. Nos résultats montrent donc que LXR régule la synthèse des acides gras polyinsaturés en plus des acides gras mono-insaturés et de la lipogenèse et que cette régulation a des conséquences sur le profil lipidique des macrophages in vitro et in vivo ainsi que sur leur réponse inflammatoire. / The nuclear receptors LXRα and LXRβ are activated by oxygenated metabolites of cholesterol. They regulate the expression of numerous genes belonging to cholesterol and fatty acids metabolism, and play a central role in inflammation and innate immunity. LXR activation inhibits atherosclerosis development, by increasing cholesterol efflux from macrophages as well as reverse cholesterol transport and biliary excretion. In addition, LXR decreases cholesterol uptake and biosynthesis. Synthetic LXR agonists fed to mice significantly decrease inflammation in atherosclerotic lesions, by inhibiting several inflammatory cytokines. However, LXR also regulate lipogenesis and monounsaturated fatty acids synthesis, and LXR agonists supplementation is accompanied by side effects due to this regulation, such as a deregulated accumulation of fatty acids in the liver and an increase in circulating LDLs. Other mecanisms still need to be characterized, such as polyunsaturated fatty acids synthesis and the consequences on cell metabolism. Our work identify a new pathway regulated by LXR, the metabolism of polyunsaturated fatty acids. The nuclear receptor LXR regulates all enzymes responsible for omega-6 and omega-3 polyunsaturated fatty acids synthesis, FADS1, FADS2 and ELOVL5. This regulation is accompanied by an increase in arachidonic acid incorporation in phospholipids, via LPCAT3 regulation, which subsequently primes human macrophages for an increased inflammatory metabolites secretion derived from arachidonic acid, such as Protaglandin E2, following a LPS stimulation. The regulation of this pathway by LXR has an effect on atherosclerosis, increasing omega-6 and omega-3 ployunsaturated fatty acids in atheroma plaques. Our results show therefore that LXR regulates polyunsaturated fatty acids synthesis in addition to monounsaturated fatty acids and lipogenesis, and that this regulation has direct consequences on lipid profile of macrophages in vitro and in vivo as well as on their inflammatory response.
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TRPV4 Implications in Inflammation and Hydrocephalic Neurological DiseaseStefanie J Simpson (6618536) 10 June 2019 (has links)
<div>Hydrocephalus is a debilitating disease characterized by an increase in cerebrospinal fluid (CSF) in the brain, leading to increases in pressure that can ultimately result in death. Current treatments for hydrocephalus include only invasive brain surgery. Therefore, the need for a pharmaceutical therapy is great. In order to develop a suitable treatment, we first must be able to study the disease and the mechanisms by which it develops. By characterizing appropriate in vivo and in vitro models, we are better able to study this disease. In this thesis, the Wpk rat model and the PCP-R cell line are described as such appropriate models. In addition to suitable models, we also require a target for drug treatment. Transient Receptor Potential Vanilloid 4 (TRPV4) is a non-selective cation ion channel present in the main CSF-producing organ in the brain, the choroid plexus (CP). Preliminary data suggest this channel plays a role in the development of hydrocephalus. In the following work, some of the mechanisms by which TRPV4 functions in the brain are also described, including through calcium-sensitive potassium channels and inflammation. From this research, we are able to achieve a better understanding of the function of TRPV4 and how it can affect the development and progression of hydrocephalus.</div>
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Impact du peptide antimicrobien issu du venin de la fourmi Tetramorium bicarinatum P17 sur la polarisation et l'acquisition des fonctions antifongiques des macrophages humains vis-à-vis de Candida albicans / Role of P17 antimicrobial peptide from the ant venom of Tetramorium bicarinatum on macrophages polarization and the acquisition of antifungal functions aganinst candida albicansBenmoussa, Khaddouj 13 January 2017 (has links)
Les peptides antimicrobiens (PAMs) cationiques sont des molécules amphipatiques conservées chez une grande diversité d'espèces vivantes. Ils participent ainsi à la défense immunitaire de nombreux organismes incluant les bactéries, les insectes, les plantes et les vertébrés. En plus de leur activité microbicide directe dirigée contre un large spectre de pathogènes, la plupart des PAMs cationiques sont désormais connus pour exercer des fonctions immunomodulatrices sur les réponses innée et adaptative. Notre équipe a récemment découvert et isolé un nouveau PAM à partir du venin de la fourmi Tetramorium bicarinatum, nommé P17. Dans ce travail, nous avons étudié les propriétés immunomodulatrices du P17 sur la réponse immunitaire innée médiée par les macrophages. Nous nous sommes plus particulièrement intéressés à sa capacité à moduler la différenciation de macrophages dérivés de monocytes humains (h-MDM) ainsi que leurs fonctions fongicides associées vis-à-vis d'une levure opportuniste majeure Candida albicans (C. albicans). Nous avons ainsi pu mettre en évidence que le P17 oriente la différenciation des h-MDM vers un phénotype alternatif caractérisé par la surexpression des récepteurs lectine de type C (CLRs) tels que Dectine-1 et le récepteur mannose (MR). De manière intéressante, nous avons mis en évidence que la surexpression de ces deux récepteurs à la surface des h-MDM activés par le P17 nécessite la mobilisation de l'acide arachidonique et la production de leucotriène B4 (LTB4). Nous avons également démontré que ce métabolite de l'AA conduit à l'activation du récepteur nucléaire PPARƴ, facteur clé de l'activation alternative des macrophages et de l'expression des CLRs associée à ce phénotype. Au cours de ce travail, nous avons démontré que les h-MDM polarisés par le P17 présentent une meilleure capacité à éliminer C. albicans. En effet, ces h-MDM activés par le P17 ont une capacité de reconnaissance, par les CLRs Dectine-1 et MR, et de phagocytose de C. albicans augmentée. De plus, l'étude des mécanismes microbicides conduisant à l'élimination de C. albicans révèle que les h-MDM activés par le P17 produisent de fortes quantités d'espèces réactives de l'oxygène (ROS) et d'IL-1ß via l'inflammasome. Ainsi, ce travail met en évidence que l'induction de l'activité fongicide des h-MDM par le P17 est dépendante de l'axe LTB4/ PPARƴ/Dectine-1-MR. Nous avons finalement confirmé ces données in vivo sur un modèle de candidose gastro-intestinale induite chez des souris traitées par voie intra-péritonéale par P17 ou non. Les résultats obtenus ont révélé que les souris traitées par P17 étaient plus résistantes à l'infection gastro-intestinale à C. albicans. La diminution de la charge fongique au niveau du cæcum des souris traitées par le P17 est associée à une meilleure efficacité de leurs macrophages à phagocyter C. albicans, à produire des ROS et à tuer C. albicans. Ainsi, ces résultats identifient le P17 comme un activateur original des propriétés antifongiques des macrophages agissant en aval de la voie permettant l'induction de l'expression des CLRs via PPARƴ. Ces données révèlent pour la première fois l'implication d'un PAM dans le contrôle de la différenciation des macrophages et leurs fonctions microbicides. / Cationic antimicrobial peptides (AMPs) are evolutionary small and amphipatic conserved molecules which are involved in the immune defense of a wide range of organisms, including bacteria, insects, plants and vertebrates. Beside their direct microbicidal activity against pathogens, most of them are known to exert immunomodulatory functions on innate and adaptive immune cells. Here we evaluated the immunomodulatory properties of an original cationic AMP, named P17, discovered and isolated by our team from the ant Tetramorium bicarinatum venom. We have focused on its efficiency to modulate human monocyte-derived macrophages (h-MDM) differentiation and its capacity to provide them an antifungal activity against the main opportunistic yeast Candida albicans (C. albicans). We showed that P17 directed h-MDM polarization toward an alternative phenotype characterized by mannose (MR) and dectin-1 C-type lectin receptors (CLRs) upregulation. Interestingly, we demonstrated that this upregulation of MR and Dectin-1 in P17-treated h-MDM requires AA mobilization and leukotriene B4 (LTB4) synthesis, essential for PPAR activation. We also demonstrated that this AA metabolite led to the PPARƴ nuclear receptor activation which is a key factor of macrophages alternative activation and the associated CLRs expression. In this study, we observed that P17-activated h-MDM exhibited an improved capacity to eliminate C. albicans. Indeed, these P17-polarized macrophages displayed an increased ability to recognize and phacocyte yeasts. Furthermore, the study of microbicidal mechanisms leading to C. albicans clearance revealed that P17-activated h-MDM produced reactive oxygen species (ROS) and inflammasome-dependant IL-1ß in high amounts. These mechanisms induction in P17-polarized h-MDM was dependent on the LTB4/ PPARƴ/Dectin-1-MR axis. Finally, these data were supported by in vivo experiments demonstrating that P17-treated mice infected with C. albicans developed less severe gastrointestinal infection related to a higher efficiency of their macrophages to engulf C. albicans, to produce ROS and to kill yeasts. Altogether, these results identify P17 as an original activator of the fungicidal response of macrophages that acts downstream the pathway leading to CLRs expression through PPARƴ activation.
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Influence of lipids (arachidonic acid and cholesterol) on calcium signalling in rodent pancreatic beta cellsYeung-Yam-Wah, Valerie 11 1900 (has links)
Ca2+ is an important mediator of stimulus-secretion coupling in beta cells of the pancreatic islets, which secrete insulin in response to elevation in plasma glucose concentration. I studied the actions of two lipids, arachidonic acid (AA) and cholesterol, on enzymatically-dissociated single beta cells of rat and mouse, using cytosolic Ca2+ ([Ca2+]i) measurement in conjunction with whole-cell patch-clamp techniques.
AA, which is produced in the beta cell upon stimulation with either glucose or acetylcholine, was found to induce a large increase in [Ca2+]i that was dependent on both extracellular Ca2+ entry and intracellular Ca2+ release. Part of the AA-mediated extracellular Ca2+ entry was due to Ca2+ influx through the arachidonate-regulated Ca2+ (ARC) channels, which have not previously been reported in beta cells. The AA-mediated intracellular Ca2+ release was a result of Ca2+ mobilization from multiple inositol trisphosphate (IP3)-sensitive intracellular stores, including the endoplasmic reticulum (ER) and an acidic Ca2+ store that is probably the secretory granules. Therefore, in beta cells, the AA-mediated Ca2+ signal may amplify the [Ca2+]i rise induced by insulin secretagogues.
Cholesterol is an integral component of cellular membranes and an important regulator of cellular functions. However, elevation of cholesterol level in the pancreatic islets reduces glucose-stimulated insulin secretion. I found that cholesterol overload impairs the glucose-stimulated [Ca2+]i increase in beta cells by two major mechanisms: the first is a decrease in glucose-stimulated ATP production, which is partly mediated by a decrease in glucose uptake, and the second is the reduction of voltage-gated Ca2+ current density. These effects of cholesterol may partly account for the decreased insulin secretion that develops in patients with type II diabetes, who typically exhibit hypercholesterolemia.
In summary, different lipids may mediate beneficial or detrimental effects on Ca2+ regulation in rodent pancreatic beta cells.
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Caractérisation structurale de la 5-lipoxygénase humaine et de son inhibition : support à la conception rationnelle d'inhibiteurs mixtes 5-LOX/COX-2/Structural characterization of human 5-lipoxygenase and its inhibition : support to the rational design of dual 5-LOX/COX-2 inhibitorsCharlier, Caroline 15 February 2006 (has links)
En bloquant les deux voies majeures de métabolisation de l’acide arachidonique, les inhibiteurs mixtes 5-LOX/COX-2 sont de puissants agents anti-inflammatoires non stéroïdiens minimisant les effets secondaires gastro-intestinaux et allergiques (asthme). Par ailleurs, ils offrent de nouvelles perspectives dans le traitement préventif de certains cancers. Contrairement à la COX-2, déjà largement étudiée, le niveau de connaissances concernant la 5-LOX humaine est beaucoup plus restreint. Notre objectif a donc été de caractériser sa structure ainsi que son mode d’interaction avec des inhibiteurs de type non redox, dans le but d’aider à la conception rationnelle d’inhibiteurs mixtes 5-LOX/COX-2. Dans un premier temps, la comparaison d’inhibiteurs 5-LOX non redox de la littérature a permis de mettre en évidence un modèle de pharmacophore à 5 points. Par ailleurs, la structure 3D de la 5-LOX humaine n’étant pas encore déterminée, nous l’avons modélisée par homologie avec la 15-LOX de lapin cristallisée et nous avons étudié, par docking, le mode d’interaction d’inhibiteurs 5-LOX non redox au sein du site actif. La combinaison des approches centrées, respectivement, sur les ligands et sur la protéine, nous a permis d’affiner l’hypothèse de pharmacophore et de proposer un modèle général d’interaction au sein du site actif 5-LOX./Dual 5-LOX/COX-2 inhibitors, acting on both major arachidonic acid metabolic pathways, are potent non-steroidal anti-inflammatory agents, with a reduced gastro-intestinal toxicity and fewer allergic adverse reactions. Moreover, they are promising in the treatment of several cancers. Whereas COX-2 has already been extensively studied, little structural or mechanistic information is available regarding human 5-LOX. Therefore, we focussed on this enzyme and characterized its 3D structure as well as its interaction with non redox inhibitors in order to help the design of dual 5-LOX/COX-2 inhibitors. Firstly, comparison of non redox 5-LOX inhibitors from the literature led to the generation of a five-point pharmacophore model. The 3D structure of human 5-LOX was then modelled based on the crystal structure of rabbit 15-LOX and, the binding modes of representative ligands were investigated through docking studies. Combination of both ligand-based and target-based approaches allowed the refinement of the pharmacophore hypothesis and led to the proposal of an interaction model for non redox inhibitors inside the 5-LOX active site.
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Influence of lipids (arachidonic acid and cholesterol) on calcium signalling in rodent pancreatic beta cellsYeung-Yam-Wah, Valerie Unknown Date
No description available.
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Differential effects of arachidonic acid and docosahexaenoic acid on cell biology and osteoprotegerin synthesis in osteoblast-like cellsCoetzee, Magdalena 09 March 2006 (has links)
The purpose of the study was to elucidate the mechanisms by which polyunsaturated fatty acids (PUFAs) prevent bone loss. MG-63 human osteoblasts and MC3T3-E1 murine osteoblasts were exposed to the n-6 PUFA arachidonic acid (AA) and the n-3 PUFA docosahexaenoic acid (DHA) as well as oestrogen (E2) and parathyroid hormone (PTH) and the effects thereof tested on a variety of biological parameters characteristic of osteoblasts. These parameters included prostaglandin E2 (PGE2) synthesis, proliferation, differentiation to mature mineralising osteoblasts as well as osteoprotegerin (OPG) and receptor activator of nuclear factor êB ligand (RANKL) secretion. Results showed that AA stimulates PGE2 production significantly in both cell lines. Stimulated PGE2 production by MC3T3-E1 cells however, was significantly higher, which might be attributed to auto-amplification by PGE2 itself in this cell line. Pre-incubation of the MG-63 cells with cyclo-oxygenase (COX)-blockers inhibited PGE2 production significantly, suggesting that both COX enzymes were involved in PGE2 synthesis. The number of functional osteoblasts is important for bone formation therefore in vitro osteoblastic cell proliferation was investigated. In contrast to the hormones E2 and PTH, both AA and DHA inhibited proliferation significantly. The AA-mediated anti-proliferative effect is possibly independent of PGE2 production, as PGE2 per se had little effect on proliferation. DHA inhibited proliferation of MG-63 cells more severely, which might be attributed to the osteosarcoma nature of the MG-63 cells. The anti-proliferative effect of these PUFAs might be attributed to modulation of cell cycle progression or anti-mitotic effects of PUFA peroxidation products. Morphological studies showed apoptotic cells after DHA exposure in MG-63 cells. There is a reciprocal relationship between reduced proliferation and the subsequent induction of cell differentiation in vitro. High basal levels of alkaline phosphatase (ALP) activity, a marker of the mature mineralising osteoblastic phenotype, were detected in MC3T3-E1 cells. Long-term exposure to AA inhibited ALP activity in these cells. This process might be PGE2-mediated. Exposure to PUFAs, however, did not compromise the ability of the MC3T3-E1 cells to differentiate to mature mineralising osteoblasts. In contrast with MC3T3-E1 cells, MG-63 cells demonstrated low basal ALP activity and were unable to differentiate to mature mineralising osteoblasts. In the absence of osteogenic-inducing supplements, PUFAs induced adipocyte-like features that might be due to the expression of high levels of PPARã in this cell line. Lipid-filled vacuoles were absent in the MC3T3-E1 cells suggesting that the MC3T3-E1 cell line may not express PPARã mRNA. The study furthermore demonstrated that PUFAs are able to modulate OPG and RANKL secretion in osteoblasts. AA inhibited OPG secretion dose-dependently in both cell lines, this could be PGE2-mediated. AA dose-dependently stimulated soluble RANKL (sRANKL) secretion in MC3T3-E1 cells thereby affecting the OPG/RANKL ratio in a negative way, supporting various reports that AA and PGE2 do cause bone resorption. No sRANKL could be detected after exposing the MC3T3-E1 cells to DHA suggesting that DHA could be protective to bone. In conclusion, contrary to in vivo evidence, this in vitro study could not indisputably demonstrate protective effects of PUFAs on the osteoblastic cell lines tested. / Thesis (PhD (Physiology))--University of Pretoria, 2006. / Physiology / unrestricted
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