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Établissement d’un nouveau modèle de souris pour étudier les cellules valvulaires interstitielles : ADAMTS19-Cre-ert2Comes, Johanna 05 1900 (has links)
Superviseur : Dr. Piet Van Vliet
Collaborateurs: Dr. Alexandre Dubrac, Dr. Martin Smith / Résumé
INTRODUCTION : Les maladies valvulaires du cœur surviennent dans 2% de la population, impliquant souvent un reflux sanguin dû au rétrécissement de la valve. Nous avons récemment identifié deux familles non apparentées étant atteintes par une sténose aortique. Le séquençage exomique des familles a révélé une mutation entrainant une perte de fonction homozygote pour le gène ADAMTS19. La relation entre la perturbation du gène ADAMTS19 et la sténose a été reproduite et donc confirmée grâce à une souris ADAMTS19-LACZ KO/KO. Cette souris montre également que ADAMTS19 est spécifiquement exprimé dans les cellules valvulaires interstitielles (VICs) dans les valves. Le rôle d’ADAMTS19 durant le développement des valves reste inconnu. Pour analyser le patron d’expression d’ADAMTS19 pendant le développement du cœur, nous avons obtenu un modèle de souris transgénique contenant une CRE-tamoxifen inductible (Cre-ERT2) qui est exprimé sous l’influence du promoteur humain ADAMTS19. HYPOTHESE/OBJECTIF : Nous émettons l’hypothèse que le promoteur humain d’ADAMTS19 inséré dans la souris ADAMTS19-Cre-ERT2 contient toutes les séquences régulatrices permettant d’exprimer le gène ADAMTS19 et que ADAMTS19 est principalement exprimé au niveau des cellules valvulaires interstitielles dans les valves. L’objectif est de caractériser le patron d’expression d’ADAMTS19 en analysant sa distribution durant le développement grâce à une souris reportrice tdTomato. Comme ADAMTS19 est spécifiquement exprimé dans les VICs, cet outil transgénique permettrait d’étudier ces cellules durant le développement. METHODE/RESULTAT : Suite à une étude in silico le promoteur ADAMTS19 est apparu comme extrêmement conservé. Par conséquent, pour analyser l’expression d’ADAMTS19 nous avons obtenu une souris BAC ADAMTS19-Cre-ERT2 contenant la séquence conservée que nous avons croisé avec une souris reportrice tdTomato. Le Tamoxifen est administré aux femelles gestantes par gavage aux jours embryonnaires E9,5, E11,5 ainsi que E13,5, et les cœurs sont extrait a E16,5. Des coupes de cœurs embryonnaires vont permettre d’identifier la localisation et la morphologie des cellules marquées. L’expression d’ADMATS19 dans les cellules valvulaires interstitielles est consistant avec le fait qu’ADAMTS19 est connu pour affecter les valves durant le développent et dans le cas de maladie valvulaire. Cependant, le patron des valves n’est pas reproductible au travers des générations. De plus, nous observons qu’ADAMTS19 est marqué dans des cellules des oreillettes et ventricule dans une lignée et dans une sous population de cellules de l’artère pulmonaire dans une autre. CONCLUSION : L’analyse des séquences de chaque lignée par séquençage permettre d’investiguer la raison de ses différents patrons et de mettre en évidence des régulateurs spécifiques. / BACKGROUND: Valvular heart disease (VHD) occurs in ~2% of the general population, often
resulting in reduced or disturbed blood flow. We recently identified two unrelated families with recessive
inheritance patterns of progressive polyvalvular heart disease in absence of any clear syndromic
phenotype. Exome sequencing revealed homozygous, rare, loss of function (LOF) alleles in both families
for the gene ADAMTS19. The relation between ADAMTS19 mutation and aortic stenosis were confirm via
an ADAMTS19-LacZ KO/KO mouse model. This model also shows that ADAMTS19 is specific of VICs
during valve development. The ADAMTS protein family includes 19 proteases that are involved in matrix
remodeling, and tissue homeostasis in development and disease. However, the role of ADAMTS19
specifically during valve development remains unknown. We aim to characterize ADAMTS19 expression
using a BAC transgenic ADMTS19-CRERT2 mouse. HYPOTHESE/OBJECTIVE We hypothesize that
the BAC used to make the ADMTS19-CRERT2 mouse contains all the regulatory elements to express it
and also that its expression will be specific to the VICs. The objective is to establish the ADAMTS19-
CREERT2 and therefore to create a new tool to study VICs in vivo. METHODS/RESULTS: In silico
analysis of the human and mouse ADAMTS19 genomic regions showed a high level of conservation.
Thus, to analyze ADAMTS19 expression patterns during mouse development, we obtained a BAC
transgenic mouse model containing a tamoxifen inducible Cre (CreERT2) that is expressed under the
influence of the human ADAMTS19 promoter and surrounding genomic region. We crossed males from
several lines created in parallel with Rosa-tdTomato reporter females to generate offspring in which
expression of the fluorescent tdTomato reporter is activated in ADAMTS19-expressing cells upon
tamoxifen administration. Surprisingly, whole mount imaging of embryos induced at E13.5 and isolated
at E16.5 revealed strong, but distinct labelling patterns in offspring from different ADAMTS19CreERT2
sublines. Whereas one line exclusively labelled VICs, consistent with ADAMTS19 in situ RNA
expression data from the Eurexpress database, another line specifically labelled cells in atrial and
ventricular, but not VICs. A third line seems to label only a subset of cells in the pulmonary artery.
Labeling of ADAMTS19-positive VICs is consistent with ADAMTS19 affecting valve development and
VHD. In addition, we observed exclusive ADAMTS19-dependent labelling in atrial and ventricular cells
or in a subset of pulmonary artery cells in two different sublines. CONCLUSION: The distinct expression
patterns in offspring from different ADAMTS19-Cre-ERT2 lines indicates that although regulation of
ADAMTS19 is conserved between human and mouse, expression in VICs versus other cells may be
dependent on mutually exclusive regulatory mechanisms.
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DUAL LOX/COX INHIBITION: A NOVEL STRATEGY TO PREVENT NEUROVASCULAR LEAKAGE IN EPILEPSYSokola, Brent S. 01 January 2018 (has links)
Epilepsy affects 3.4 million patients in the USA and is characterized by recurring seizures. The blood-brain barrier is leaky in epilepsy and may contribute to seizure progression but the mechanisms which cause this leakage are not fully understood. We hypothesized that seizures trigger LOX- and COX-mediated blood-brain barrier leakage and that dual LOX/COX inhibition prevents barrier leakage in vivo. To test this hypothesis, we administered either the dual LOX/COX inhibitor licofelone or a combination of the 5-LOX inhibitor zileuton and the COX-2 inhibitor celecoxib to rats that experienced status epilepticus (SE). Serum and brain capillaries were isolated 48 hours after SE and serum S100β levels were measured and Texas Red™ leakage rates were determined. Dual inhibition of 5-LOX and COX prevented serum S100β elevations observed in SE rats in a dose-dependent manner with licofelone. Inhibition of 5-LOX and COX-2 with zileuton and celecoxib completely prevented serum S100β elevation. Texas Red™ leakage rates for SE rats were also reduced in a dose-depended manner with licofelone and reduced to control rates with zileuton and celecoxib. These data support our hypothesis that seizure-induced blood-brain barrier leakage is mediated by LOX and COX, and inhibition of these enzymes prevents barrier leakage.
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Optimization of PCR protocols used for genotyping transgenic mice & Evaluation of a method for co-detecting mRNA and protein / Optimering av PCR-protokoll som används för genotypning av transgena möss och utvärdering av en metod för att detektera mRNA och proteinIsaksson, Amanda January 2017 (has links)
The aim of the current study was divided into two separate goals, (i) optimization of a number of PCR-based protocols employed for genotyping transgenic mouse lines and (ii) evaluating a protocol for co-detection of mRNA and its correlated protein in the mouse midbrain. The optimization was performed on PCR protocols for genotyping the following transgenic mouse lines; Dat-Cre, Vglut2-Lox, Vglut2-Cre and Vmat2-Lox. Also, two different polymerases were evaluated parallel to each other – KAPA and Maxima Hot Start. One of the main findings from the PCR optimizations were that for the Vglut2-Lox protocol. By decreasing the annealing temp and increasing the MgCl2 the bands appeared brighter. For the second part of the project, in-situ hybridization (ISH) was used to detect the mRNA expression with a `non-radioactive in situ hybridization´ protocol, using digoxigenin or fluorescein labelled riboprobes (mRNA probes). To detect the correlated protein a basic immunohistochemistry (IHC) protocol with the use of primary and secondary antibodies was implemented. The combined protocol was tested with Nd6 and Grp markers. Before testing to combined the protocols the ISH protocol was performed alone with riboprobes for Girk2, Lpl and Fst. The combined protocol detected mRNA and protein for both the control marker Th and the Nd6 marker. In conclusions, the optimized PCR protocols were optimal when used with the Maxima Hot Start polymerase and the new combined ISH and IHC protocol worked for markers Th and Nd6.
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An In-vivo Analysis of SLMAP Function in the Postnatal Mouse MyocardiumRehmani, Taha January 2017 (has links)
SLMAP is a tail anchored membrane protein that alternatively splices to generate three isoforms, SLMAP1, SLMAP2 and SLMAP3. Previous studies in our lab have shown that the postnatal cardiac-specific overexpression of SLMAP1 results in intracellular vesicle expansion and enhanced endosomal recycling. I generated a postnatal cardiac-specific knockout model using the Cre-Lox system to nullify all three SLMAP isoforms and further evaluate its role in the mouse myocardium. SLMAP knockdown and knockout mouse hearts were analyzed with western blotting and qPCR. I found that only SLMAP3 was nullified and phenotypic evaluation through echocardiography indicated that young and old SLMAP3 knockout animals showed no remarkable changes in cardiac function. Furthermore, challenge with stressor isoproterenol had a similar response to wildtype and knockout mice in cardiac structure and function. Surprisingly the level of expression of SLMAP1 and SLMAP2 was maintained in the myocardium from SLMAP3 deficient mice. Interestingly the machinery involved in endosomal recycling was not impacted by the loss of SLMAP3. These data indicate that loss of SLMAP3 does not alter cardiac structure and function in the postnatal myocardium in the presence of SLMAP1 and SLMAP2.
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Preferential arborization of dendrites and axons of parvalbumin- and somatostatin-positive GABAergic neurons within subregions of the mouse claustrum / マウス前障においてパルブアルブミン陽性およびソマトスタチン陽性GABA作動性神経細胞が示す、亜領域に選択的な樹状突起及び軸索の走行Takahashi, Megumu 23 March 2023 (has links)
京都大学 / 新制・課程博士 / 博士(医学) / 甲第24505号 / 医博第4947号 / 新制||医||1064(附属図書館) / 京都大学大学院医学研究科医学専攻 / (主査)教授 渡邉 大, 教授 林 康紀, 教授 井上 治久 / 学位規則第4条第1項該当 / Doctor of Medical Science / Kyoto University / DFAM
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Lipidomics of polyunsaturated fatty acid-derived oxygenated metabolitesNicolaou, Anna, Massey, Karen A. January 2011 (has links)
No / Nutritionally important PUFAs (polyunsaturated fatty acids) mediate some of their bioactivities through formation of oxygenated metabolites. These bioactive lipids are formed by COX (cyclo-oxygenase), LOX (lipoxygenase) and cytochrome-P450-catalysed reactions, as well as non-enzymatic lipid peroxidation. These reactions produce numerous species, some of which can be formed through more than one pathway. MS-based lipidomics offers the selectivity and sensitivity required for qualitative and quantitative analysis of multiple lipid species, in a variety of biological systems, and can facilitate the study of these mediators.
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Le rôle de la 12/15-Lipoxygénase dans la pathogenèse de l'arthroseHabouri, Loures 04 1900 (has links)
No description available.
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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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Role of the Heterotrimeric Go Protein Alpha-subunit on the Cardiac Secretory PhenotypeRoeske, Cassandra 21 May 2013 (has links)
Atrial natriuretic factor (ANF) is a polypeptide hormone produced in heart atria, stored in atrial secretory granules and released into the circulation in response to various stimuli. Proper sorting of ANF at the level of the trans-Golgi network (TGN) is required for the storage of ANF in these specific granules, and this sorting of hormones has been found to be associated with G-proteins. Specifically, the Go protein alpha-subunit (Gαo) was established to participate in the stretch-secretion coupling of ANF, but may also be involved in the transporting of ANF from the TGN into atrial granules for storage and maturation. Based on knowledge of Gαo involvement in hormone production in other endocrine tissues, protein-protein interactions of Gαo and proANF and their immunochemical co-localization in granules, the direct involvement of these two proteins in atrial granule biogenesis is probable. In this study, mice were created using the Cre/lox recombination system with a conditional Gαo knockout in cardiocytes to study and characterize ANF production, secretion and granule formation. Deletion of this gene was successful following standard breeding protocols. Characterization and validation of cellular and molecular content of the knockout mice through mRNA levels, protein expression, peptide content, electron microscopy, and electrocardiography determined that a significant phenotypic difference was observed in the abundance of atrial granules. However, Gαo knockout mice did not significantly alter the production and secretion of ANF and only partially prevented granule biogenesis, likely due to incomplete Gαo knockout. These studies demonstrate an involvement of Gαo in specific atrial granule formation.
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Etude de la détonation dans un jet diphasique cryogénique GH2-LOx : contribution aux études sur les moteurs à onde de détonation / Detonation study of a cryogenic two-phase H2-O2 mixture : detonation wave engines contributionJouot, Fabien 30 November 2009 (has links)
L’objectif de cette thèse est d’étudier l’initiation directe et la propagation d’une détonation dans un milieu cryogénique diphasique GH2-LOx dans le cadre général des moteurs à onde de détonation pour la propulsion spatiale. Un rappel des bases théoriques sur les processus d’atomisation d’un jet liquide, puis sur la détonation en phase gazeuse, et enfin sur la détonation dans un mélange diphasique, constituent le premier chapitre de la thèse. Le deuxième chapitre présente les dispositifs expérimentaux et les techniques utilisés pour mener à bien les expériences de caractérisation du jet diphasique et d’étude de la détonation. Le troisième chapitre est consacré à l’étude dans un tube en quartz de la granulométrie d’un jet diphasique GHe-LOx non réactif. Une cartographie est ainsi réalisée sur l’ensemble du tube, pour différents débits d’injection. Ces résultats sont corroborés par une étude théorique sur une goutte isolée et par une étude numérique sur le comportement du jet en champ proche de l’injecteur. Le quatrième chapitre présente les résultats de l’étude de la détonation dans un tube en acier d’un mélange réactif GH2-LOx. La détonation est étudiée en fonction de divers paramètres : énergie d’initiation stockée, emplacement du dispositif d’initiation par étincelle, richesse globale du mélange. La célérité et la pression de détonation, ainsi que la structure tridimensionnelle de la détonation, sont les principales informations recueillies pour l’étude du phénomène de détonation en mélange diphasique. Une étude théorique des caractéristiques de la détonation apporte des éclairages supplémentaires sur la détonation à très basse température (100 K). / Within the general framework of detonation engines for space propulsion purpose, this work aims to study direct initiation and propagation of detonation in a cryogenic twophase GH2-LO2 mixture. First chapter is constituted by theoretical basis and state of art on atomization processes in liquid jets, then on gas-phase detonation, and finally on two-phase detonation. Second chapter describes experimental set-up and associate techniques in order to carry out two-phase jet characterization and detonation study. Third chapter is dedicated to the study of droplet size distribution of non reactive two-phase GHe-LO2 jet in a quartz tube. Thus, a droplet size map is constituted through the whole tube, for different helium injection speeds. These results are compared with theoretical study dealing with vaporization and movement of a droplet and with numerical simulations on jet behavior close to the injector. Fourth chapter presents results of a detonation study of a reactive GH2-LO2 two-phase mixture in a semi-open tube. Detonation is studied as a function of following parameters: initiation energy, spark initiation device location along the tube, global equivalence ratio. Velocity, peak pressure and three-dimension structure detonation are the main data collected to study two-phase detonation phenomena. A theoretical study of detonation characteristics brings additional information on detonation at low temperature (100 K).
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