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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
11

Potential role of non-enzymatic glycation and glycoxidation of low density lipoprotein in diabetic atherosclerosis

Lam, Chi-wai, 林智威 January 2002 (has links)
published_or_final_version / Medicine / Master / Master of Philosophy
12

Comparison of structure and function of lipoprotein receptors

Norman, Dennis January 1999 (has links)
No description available.
13

Studies of shock propagation and thermal smoothing in laser irradiated foam targets

Iwase, Akio January 1999 (has links)
No description available.
14

The role of metal ions in LDL peroxidation

Crabtree, Elaine January 1997 (has links)
No description available.
15

Susceptibilité de la muqueuse intestinale aux xénobiotiques : implication dans la physiopathologie des maladies inflammatoires chroniques de l’intestin (MICI) : exemple du gène Rac1 / Susceptibility of intestinal mucosa to xenobiotics : role in the physiopathology of inflammatory bowel diseases (IBD) : example of Rac1 gene

Bourgine, Joanna 24 October 2011 (has links)
Les Maladies Inflammatoires Chroniques de l’Intestin (MICI) regroupent la maladie de Crohn (MC) et la Rectocolite Hémorragique (RCH), deux maladies qui se caractérisent par l’inflammation de la paroi d’une partie du tube digestif, source de lésions destructrices (ulcérations). Ces pathologies complexes sont influencées par de multiples facteurs génétiques et environnementaux. D’une part, de nombreux gènes de susceptibilité pour ces maladies ont été identifiés, mais ils ne permettent d’expliquer qu’une fraction mineure du développement des MICI. D’autre part, certaines études montrent qu’un dysfonctionnement du processus de prise en charge des xénobiotiques dans la muqueuse digestive peut jouer un rôle dans l’initiation et/ou la progression des MICI. Notre travail a consisté, dans un premier temps, en l’étude du profil d’expression de gènes codant pour des protéines impliquées dans le métabolisme et le transport des xénobiotiques. Une stratégie de RT-PCR quantitative en temps réel, permettant l’analyse simultanée de l’expression de 377 gènes, a été utilisée. Cette analyse a été réalisée sur des échantillons de muqueuse intestinale de sujets témoins et de patients atteints de MC, ainsi que sur cinq lignées de cellules épithéliales intestinales.Cette étude a permis d’identifier les systèmes de prise en charge des xénobiotiques présents dans la muqueuse intestinale saine. Des profils d’expression différents ont été mis en évidence entre les tissus intestinaux sains et inflammatoires, mais également entre les tissus intestinaux et les lignées cellulaires intestinales, ce qui suggère des différences majeures dans les processus de prise en charge cellulaire des xénobiotiques, et, par conséquent des différences de susceptibilité à l’effet des composés toxiques exogènes. Dans un second temps, la petite protéine G, Rac1, a été étudiée. Cette protéine est impliquée dans la réparation des ulcérations de l’épithélium intestinal et a récemment été identifiée comme la cible des métabolites actifs des médicaments thiopuriniques, largement prescrits dans le traitement des MICI. La nature et l’étendue de la variabilité de la séquence nucléotidique du gène Rac1 a été évaluée, chez des volontaires sains et des patients atteints de MICI, à l’aide d’une stratégie basée sur le couplage de l’analyse du polymorphisme de conformation de fragments d’ADN simple brin générés par réaction de polymérisation en chaine (PCR-SSCP) et du séquençage. Des études in silico et in vitro des conséquences fonctionnelles des polymorphismes d’intérêts ont ensuite été effectuées dans des lignées cellulaires intestinales (HT29 et Caco-2) et lymphocytaires (Jurkat). Cela nous a conduits à mieux caractériser le promoteur de Rac1 par une analyse de délétion séquentielle et par des techniques de ChIP et d’EMSA.Cette étude nous a permis de démontrer pour la première fois l’existence de polymorphismes génétiques fonctionnels de Rac1 et d’identifier son promoteur minimal, ainsi que des facteurs de transcription à l’origine de la régulation de cette protéine. / Crohn’s disease (CD) and Ulcerative colitis (UC) are chronic inflammatory bowel diseases (IBD) of the gastrointestinal tract. These are multifactorial polygenic diseases with probable genetic heterogeneity. An emerging concept suggesting that dysfunction(s) of the processing of xenobiotics in the intestinal mucosa may be an important event in the initiation and progression of IBD has been discussed. Firstly, in this study, a precise and reliable characterization of the global expression profile of genes which code enzymes, transporters and nuclear factors involved in the processing of xenobiotics has been performed in intestinal epithelium of controls or patients with IBD, and in 5 intestinal cell lines. A quantitative real-time RT-PCR analysis using TaqMan Low Density Arrays (TLDA) was performed to simultaneously measure the expression of 377 genes.This work has identified genes encoding proteins that are involved in the metabolism and the disposition of xenobiotics in the healthy intestinal mucosa. Different genes expression profile between healthy and inflammatory intestinal tissues and between healthy intestinal tissues and intestinal cell lines were found. These tissues will consequently display distinctive susceptibility toward environmental chemicals and their toxic effects.Secondly, the small G protein, Rac1, which regulates cutaneous and mucosal intestinal wound healing and is identified as a target of active metabolites of thiopurine drugs, used in the treatment of IBD, has been studied. We searched for sequence variations by analysing the nucleotide sequence of the promoter and the coding sequence of Rac1 in genomic DNA from healthy volunteers and patients with IBD, using a PCR-single strand conformation polymorphism (SSCP) strategy and sequencing. The functional consequences of variations, that have been identified, were then analysed in silico and in vitro, in human intestinal cell lines (HT29 and Caco-2) and leukemia T-lymphocyte cell line (Jurkat). Via various deletion constructs, a putative regulatory region was identified and characterized further by chromatin immunoprecipitation and electrophoretic mobility shift assays.This work provides the first evidence that a functional genetic polymorphism of Rac1 activity exists. Furthermore, this study characterizes the proximal promoter of Rac1 gene and demonstrates the presence of consensus binding sites for numerous transcription factors, which could influence gene expression.
16

Oxidiertes LDL und sein Bestandteil Lysophosphatidylcholin potenzieren die Angiotensin-II vermittelte Vasokonstriktion über Stimulation von RhoA / Oxidized LDL and the component lysophosphatidylcholine are potentiating the angiotensin-II induced vasoconstriction through activation of rhoA

Mameghani, Alexander Tapio January 2009 (has links) (PDF)
RhoA stimuliert den Vasotonus durch eine Ca2+-Sensitivierung der glatten Muskelzellen, z.B. bei der Hypercholesterinämie oder Atherosklerose. Diese Studie untersuchte den Einfluss von oxidierten Lipoproteinen (OxLDL), die in atherosklerotischen Läsionen akkumulieren, auf den durch Angiotensin II (Ang II) erhöhten Vasotonus an isolierten Kaninchenaorten mit besonderem Augenmerk auf den RhoA/RhoA-KLinase-Signalweg. Zunächst wurde die Dilatationsfähigkeit des Endothels nach Vorinkubationen mit Ang II und Erhöhung des oxidativen Stresses überprüft und gezeigt, dass auch nach mehrstündiger Behandlung mit hohen Dosen des Vasokonstriktors die Endothel-abhängige Dilatationsfähigkeit voll erhalten blieb. OxLDL hatte keinen Einfluss auf den Vasotonus eines unstimulierten Gefäßes, potenzierte aber die Kontraktionsantwort durch Ang II. Dieser Effekt wurde durch die Behandlung mit Calyculin A und Staurosporin abgeschwächt. Eine RhoA-Kinase-Inhibition mit Y27632 hat den OxLDL-Effekt vollkommen aufgehoben und die RhoA-Inhibition durch die C3-ähnliche Transferase von Clostridium limosum deutlich abgeschwächt um ca. 50%. Lysophosphatidylcholin (LPC), ein Bestandteil von OxLDL, ruft denselben Effekt hervor wie OxLDL auf die Kontraktionsantwort von Ang II-stimulierten Aorten und dieser wird ebenso durch Y27632 vollkommen antagonisiert, wie durch die C3-ähnliche Transferase partiell vermindert. OxLDL und sein Bestandteil LPC vermitteln Ihren Effekt durch eine Stimulation des RhoA/RhoA-Kinase-Signaltransduktionsweg, was in atherosklerotischen Gefäßen zur Entstehung von Vasospasmen beitragen kann. / RhoA stimulates the vascular tone via a Ca2+-sensitizing of smooth muscle cells, for e.g. in case of hypercholesterinemia or atherosclerosis. This study has investigated the influence of oxidized low-density-lipoproteins (OxLDL), which are accumulated in atherosclerotic lesions, on angiotensin-II (Ang II) induced vasoconstriction in isolated aortic rings of rabbits. We focused on the rhoA/rhoA-kinase-pathway. First we showed that treatment for hours with AngII and inductors of oxidative stress had no effect on the endothel-derived vasodilation. OxLDL alone had no effect on the vasodilatation, but it potentiates the vasoconstriction that was induced by Ang II. In absence of Ang II there was no vasoconstriction response of vascular smooth muscle if OxLDL was co-incubated. The effect of OxLDL is partially diminushed by calyculin A and staurosporine. Inhibition of rhoA-kinase by Y27632 led to a complete reduction of the OxLDL-effect and inhibition of rhoA by a C3-like transferase of clostridium limosum resulted in a 50% decrease. Lysophosphatidylcholine (LPC), a component of OxLDL, had the same effect on vasoconstriction and vasodilator-response as OxLDL. Treatment with Y27632 and the C3-like transferase modulated the effect of LPC the same way. OxLDL and the component LPC are taking influence on the rhoA/rhoA-kinase-pathway. This can be a cause of increase vascular tone in atherosclerotic lesions.
17

Role of lectin-like oxidized low density lipoprotein receptor-1 (LOX-1) in diabetes mellitus

Shiu, Wing-ming, Sammy., 邵永明. January 2012 (has links)
Lectin-like oxidized low density lipoprotein receptor-1 (LOX-1) is a recently identified scavenger receptor expressed in endothelial cells and mediates the uptake of oxidized LDL (oxLDL). LOX-1 expression is increased in atherosclerotic lesions in animals and humans. Recent evidence has suggested that LOX-1 is involved in the development and progression of atherosclerosis. In addition to endothelial cells, it has also been reported that LOX-1 is also expressed by other cell types like macrophages. It is a multi-ligand class E scavenger receptor and cellular expression of LOX-1 can be induced by many of its ligands. The concentration of some of these ligands like oxLDL and advanced glycation end products (AGEs) are increased in the diabetic milieu. My hypothesis is that LOX-1 expression is increased in diabetes mellitus and LOX-1 activation may play a role in the development of micro- and/or macrovascular complications of diabetes. The objective of this thesis is to elucidate the role of LOX-1 in type 2 diabetes mellitus and its complications. The effect of modified LDL and AGEs on LOX-1 expression and the cellular response upon LOX-1 activation was investigated. In vitro studies have shown that both AGEs and oxLDL can activate and increase cellular expression of LOX-1 and the soluble form of LOX-1 (sLOX-1) in cultured endothelial cells. In addition, LDL modified by glycoxidation, is also a ligand of LOX-1 and glycoxidized LDL is even more potent than oxLDL in inducing LOX-1 expression. In patients with type 2 diabetes, serum level of sLOX-1 was significantly higher than non-diabetic normal control, indicating that LOX-1 expression was increased in diabetes. Serum levels of AGEs and glycoxidized LDL were important determinants of serum sLOX-1 level, and lowering serum AGEs led to a beneficial reduction in serum sLOX-1 concentration. Hence, AGEs was clearly an important ligand of LOX-1 in diabetes mellitus, and experiments were performed to further elucidate the underlying signaling pathway involved in the up-regulation of LOX-1 by AGEs. This was mediated by ligation of AGEs to the receptor for advanced glycation end products (RAGE) and activation of phosphoinositide 3-kinase. Mammalian target of rapamycin was a found to be a key downstream intermediary in AGEs-inducible LOX-1 expression in endothelial cells. I further demonstrated that LOX-1 was also expressed in human renal mesangial cells, and expression was at a low level at basal state but inducible by its ligands. Up-regulation of LOX-1 expression in activated mesangial cells resulted in increased oxidative stress, as well as increased production of proinflammatory cytokines, chemokines and growth factors. These experimental findings would suggest that LOX-1 might potentially be involved in renal inflammation and diabetic nephropathy. The above results collectively suggest that diabetes is associated with increased LOX-1 activation, and LOX-1 may play a role in the development of diabetic complications. Hence, LOX-1 might represent a suitable target for the future development of new strategies for treating and preventing diabetic vascular complications. / published_or_final_version / Medicine / Doctoral / Doctor of Philosophy
18

Abnormalities of low-density lipoprotein metabolism in patients with coronary artery disease.

Shi, Fang. January 1991 (has links)
Studies have shown that hypercholesterolemia is a risk for cardiovascular disease; however, some normocholesterolemic individuals still develop coronary atherosclerosis. This project was undertaken to investigate the association of abnormalities of low density lipoprotein (LDL) metabolism, in the absence of hypercholesterolemia, with the development of coronary artery disease (CAD). Mononuclear leukocytes (MNL), HL-60 cells and 1,25-dihydroxyvitamin D₃-induced HL-60 macrophages were used as model systems to study the effect of an altered LDL composition on cellular lipoprotein and sterol metabolism. LDL and MNL were isolated from patients with and without CAD. The mean rate of LDL degradation was 1.7-fold higher in CAD-MNL than in control-MNL (P < 0.05), independent of the LDL source. The increased LDL degradation rate in CAD-MNL appeared to be due to an increased LDL receptor activity of CAD-MNL and not to an increased CAD-LDL interaction with the receptor since LDL isolated from patients with and without CAD had similar in vitro degradation rates by HL-60 cells and D₃-induced HL-60 macrophages. LDL from CAD patients (CAD-LDL) contained significantly less cholesteryl ester per particle than LDL from control subjects (Control-LDL). The ability of CAD-LDL and Control-LDL to regulate sterol and lipoprotein metabolism was compared in HL-60 cells. The results indicate that CAD-LDL exhibited reduced abilities to suppress receptor-mediated LDL degradation and to activate acyl-CoA:cholesterol acyltransferase as compared to Control-LDL. There was no significant difference in the rate of sterol synthesis between cells treated with CAD-LDL and Control-LDL. The data support the hypothesis that cholesteryl ester-poor CAD-LDL exhibits a decreased ability to down-regulate LDL receptor activity which could in part account for the observed increase in LDL degradation by MNL from CAD patients. A noncompetitive enzyme-linked immunosorbent assay (ELISA) was developed to measure plasma apolipoproteins (apo) A-I and B. The results indicate that a reduced plasma apo A-I level was associated with CAD patients even if there were no significant differences in the levels of high density lipoprotein cholesterol when compared with individuals without CAD.
19

Untersuchungen zur Abhängigkeit der oxidativen Low Density Lipoprotein (LDL)-Modifikation von der 15-Lipoxygenaseexpression in monozytären Zellen /

Zalán, Ildikó. January 1994 (has links) (PDF)
Univ., Diss.--Heidelberg, 1994.
20

Ozoniertes Low Density-Lipoprotien (OzLDL)

Cappello, Christian January 2009 (has links)
München, Techn. Univ., Diss., 2009.

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