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Lipoprotein particles associate with lipid-linked proteins and are required for long-range Wingless and Hedgehog signaling / Lipoprotein-Partikel assoziieren mit lipid-modifizierten proteinen und sind notwendig zur Wingless-und Hedgehog Signaltransduktion über grosse Distanzen.Panakova, Daniela 21 June 2005 (has links) (PDF)
Morphogens of the Wnt and Hedgehog families are secreted signaling molecules that coordinate growth and patterning of many different tissues. Both, Wingless and Hedgehog spread across long distances in developing wing of Drosophila melanogaster. However, both proteins are covalently modified with lipid moieties. The mechanisms that allow long-range movement of such hydrophobic molecules are unclear. Like Wingles and Hedgehog, glycosylphosphatidylinositol (gpi)-linked proteins also transfer between cells with their lipid anchor intact. It has been speculated that gpi-linked proteins and lipid-linked morphogens travel together on a membranous particle, which was termed an argosome. As yet however, no functional link between argosome production and dispersal of lipid-linked proteins has been established. The topic of this thesis is to understand the cell biological nature of the argosome and thus contribute to understanding of morphogen gradient formation. To address the question of argosome biosynthesis, at least two models have been proposed. One possibility is that argosomes are membranous exovesicles with a complete membrane bilayer. Alternatively, argosomes might resemble lipoprotein particles that comprise on of a family of apolipoproteins scaffolded around a phospholipid monolayer that surrounds a core of esterified cholesterol and triglyceride. Lipid-modified proteins of the exoplasmic face of the membrane (like GFPgpi, Wingless or Hedgehog) might fit well into the outer phospholipid monolayer of such a particle. Here, I utilize biochemical fractionation to determine the sort of particle that lipid-linked proteins associate with. I show that Wingless, Hedgehog and gpi-linked proteins bind Drosophila lipoprotein particles in vitro, and colocalize with them in wing imaginal discs. Next, I use genetic means to address the functional importance of this association. I demonstrate that reducing Lipophorin levels in Drosophila larvae perturbs long-range but not shor-range Wingless and Hedgehog signaling, and increases the sequestration of Hedgehog by Patched. I propose that Lipophorin particles are vehicles for the long-range movement of lipid-linked morphogens and gpi-linked proteins.
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Metabolism of triacylglycerol-rich lipoproteins in sheepMason, Susan Leigh January 1991 (has links)
This thesis describes two approaches for studying of lipoprotein metabolism in sheep. The first approach involves the assay of lipoprotein lipase (LPL) activity to determine the role of lipoprotein-triacylglycerol fatty acids in fat deposition in sheep. This enzyme is the rate limiting enzyme in the hydrolysis of fatty acids from lipoprotein-triacylglycerol. The second approach was to characterize and quantify in vivo lipoprotein metabolism using iodinated very low density lipoprotein (¹²⁵I-VLDL) and low density lipoprotein (¹³¹I-LDL). Cross-bred lambs were divided into two treatment groups and either weaned early at 5 weeks of age or remained suckling. Lambs were slaughtered at 12 or 23 weeks at which time the body composition and adipose tissue LPL activity were determined. The differences in rearing led to differences in body composition. The suckled lambs were larger and fatter than weaned lambs. The increased fatness in the suckled lambs was associated with increased LPL activity (U/mg protein) in subcutaneous adipose tissue and was reflected in higher LPL activity in post-heparin plasma (PHP) taken 2 days prior to slaughter. The role of insulin in the regulation of LPL activity was investigated by either infusing a subset of the weaned and suckled lambs with insulin for 7 or 18 weeks or using the euglycemic clamp technique to study the effect of short insulin infusions. The long term infusion of insulin had no significant effect on PHP LPL or on adipose tissue LPL (U/g tissue). However, after infusing insulin for 6h at 6.3 mU.kg⁻·⁷⁵.h⁻¹ during the euglycemic clamps, a two fold increase in LPL activity in biopsied subcutaneous adipose tissue was observed. In the second approach, in vivo lipoprotein metabolism was investigated in 4 lambs using apolipoprotein B as a marker. Following the simultaneous injection of ¹²⁵I VLDL and ¹³¹I VLDL, the specific activities of apoB in VLDL, IDL and LDL fractions were determined. ApoB specific activity curves demonstrated that VLDL is metabolised to IDL and subsequently to LDL. The turnover of VLDL-B (3.45mg.d⁻¹.kg⁻¹) and LDL-B (4.8mg.d⁻¹.kg⁻¹) was calculated by fitting the VLDL-¹²⁵I-B and LDL-¹³¹I-B specific activity data to a mono-exponential equation. The metabolism of lipoproteins, inferred from the study of apoB, was shown to be similar in sheep to that reported in other animals although the amount of lipoprotein synthesised was low. A model to describe the kinetics of apoB metabolism in sheep was developed using SAAM. The proposed model features a three pool delipidation chain for VLDL, and subsystems containing two pools for IDL and LDL. IDL may be catabolised to LDL or cleared directly from the plasma. The developed model can now be used to compare the metabolism of lipoproteins in different physiological states and to design new experiments to study lipoprotein metabolism further.
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Lipoprotein particles associate with lipid-linked proteins and are required for long-range Wingless and Hedgehog signalingPanakova, Daniela 01 July 2005 (has links)
Morphogens of the Wnt and Hedgehog families are secreted signaling molecules that coordinate growth and patterning of many different tissues. Both, Wingless and Hedgehog spread across long distances in developing wing of Drosophila melanogaster. However, both proteins are covalently modified with lipid moieties. The mechanisms that allow long-range movement of such hydrophobic molecules are unclear. Like Wingles and Hedgehog, glycosylphosphatidylinositol (gpi)-linked proteins also transfer between cells with their lipid anchor intact. It has been speculated that gpi-linked proteins and lipid-linked morphogens travel together on a membranous particle, which was termed an argosome. As yet however, no functional link between argosome production and dispersal of lipid-linked proteins has been established. The topic of this thesis is to understand the cell biological nature of the argosome and thus contribute to understanding of morphogen gradient formation. To address the question of argosome biosynthesis, at least two models have been proposed. One possibility is that argosomes are membranous exovesicles with a complete membrane bilayer. Alternatively, argosomes might resemble lipoprotein particles that comprise on of a family of apolipoproteins scaffolded around a phospholipid monolayer that surrounds a core of esterified cholesterol and triglyceride. Lipid-modified proteins of the exoplasmic face of the membrane (like GFPgpi, Wingless or Hedgehog) might fit well into the outer phospholipid monolayer of such a particle. Here, I utilize biochemical fractionation to determine the sort of particle that lipid-linked proteins associate with. I show that Wingless, Hedgehog and gpi-linked proteins bind Drosophila lipoprotein particles in vitro, and colocalize with them in wing imaginal discs. Next, I use genetic means to address the functional importance of this association. I demonstrate that reducing Lipophorin levels in Drosophila larvae perturbs long-range but not shor-range Wingless and Hedgehog signaling, and increases the sequestration of Hedgehog by Patched. I propose that Lipophorin particles are vehicles for the long-range movement of lipid-linked morphogens and gpi-linked proteins.
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Regulation of outer surface lipoprotein A in the Lyme disease spirochete Borrelia burgdorferiOman, Tara Lynn 07 October 2013 (has links)
Indiana University-Purdue University Indianapolis (IUPUI) / Borrelia burgdorferi, a bacterium which causes Lyme disease, is maintained in nature through a cycle involving two distinct hosts: a tick vector and a mammalian host. To adapt to these two diverse environments, B. burgdorferi undergoes dramatic alterations in its surface lipoprotein. Two essential lipoproteins, outer surface protein A (OspA) and outer surface protein C (OspC), are reciprocally regulated throughout the B. burgdorferi lifecycle. Very little is known about the regulation of OspA. These studies elucidate the regulatory mechanisms controlling the expression of OspA. Various truncations of the ospA promoter were created and then studied in our novel in vitro model of ospA repression or grown within the host-adapted model. A T-Rich region of the ospA promoter was determined to be a cis-element essential for both the full expression and full repression of ospA.
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Molecular Regulators Of Post-golgi Vldl Transport Vesicle (pg-vtv) BiogenesisRiad, Aladdin 01 January 2013 (has links)
Amongst its numerous functions, the liver is responsible for the synthesis and secretion of very low-density lipoprotein (VLDL). VLDL particles play the important role of facilitating the transport of lipids within the aqueous environment of the plasma; yet high plasma concentrations of these particles result in the pathogenesis of atherosclerosis, while low VLDL secretion from the liver results in hepatic steatosis. VLDL synthesis in the hepatocyte is completed in the Golgi apparatus, which serves as the final site of VLDL maturation prior to its secretion to the bloodstream. The mechanism by which VLDL’s targeted transport to the plasma membrane is facilitated has yet to be identified. Our lab has identified this entity. Our findings suggest that upon maturation, VLDL is directed to the plasma membrane through a novel trafficking vesicle, the Post-Golgi VLDL Transport Vesicle (PG-VTV). PG-VTVs containing [3H] radiolabeled VLDL were generated in a cell-free in vitro budding assay for study. First, the fusogenic capabilities of PG-VTVs were established. Vesicles were capable of fusing with the plasma membrane and delivering the VLDL cargo for secretion in a vectorial manner. The next goal of our study is to characterize key regulatory molecular entities necessary for PG-VTV biosynthesis. A detailed analysis was undertaken to determine the PG-VTV proteome via western blot and two-dimensional difference in gel electrophoresis. The identification of key molecular regulators will potentially offer therapeutic targets to control VLDL secretion to the bloodstream.
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Characterization of the interaction between acetylcholinesterase and laminin : a template for discovering redundancySwart, Chrisna 03 1900 (has links)
Thesis (PhD)--Stellenbosch University, 2012. / ENGLISH ABSTRACT: Apart from its primary function in the synaptic hydrolysis of acetylcholine,
acetylcholinesterase (AChE) has been shown through in vitro demonstrations to be able
to promote various non-cholinergic functions, including cell adhesion and neurite
outgrowth, differentiation, and amyloidosis. AChE was also shown to bind to mouse
laminin-111 in vitro by an electrostatic mechanism. Previous results suggest that the site
on AChE recognised by certain monoclonal antibodies (MAbs) might be critical for
differentiation. These MAbs were found to inhibit both laminin binding and cell adhesion
in neuroblastoma cells. In this study, the structure and characteristics of this site were
investigated, using the AChE-laminin interaction as a template as well as a detailed
epitope analysis of the MAbs. The interaction sites of AChE and laminin were
investigated using phage display, modelling and docking, synthetic peptides, enzyme
linked immunosorbent assays (ELISAs) and conformational interaction site mapping.
Docking of AChE with the single-chain variable fragments (scFvs) produced from the
phage display showed the major recognition motifs to be the 90Arg-Glu-Leu-Ser-Glu-Asp
motif, the 40Pro-Pro-Met-Gly sequence, and the 59Val-Val-Asp-Ala-Thr-Thr (human)
motif. Mouse AChE was found to interact with the basic structures Val2718-Arg-Lys-Arg-
Leu2722; Tyr2738-Tyr2739, Tyr2789-Ile-Lys-Arg-Lys2793; and Val2817-Glu-Arg-Lys2820, on the
1 G4 domain of laminin. ELISAs using synthetic peptides confirmed the involvement of
the AG-73 site (2719-2729). This site overlaps with laminin’s heparin-binding site.
Docking showed the major component of the interaction site on AChE to be the acidic
Arg90-Glu-Leu-Ser-Glu-Asp95 (omega loop), and also involving the Pro40-Pro-Val42,
Arg46 (linked to Glu94 by a salt bridge) and the hexapeptide Asp61 Ala-Thr-Thr-Phe-Gln66.
Epitope analysis showed the MAb’s major recognition site to be the sequence Pro40-Pro-
Met-Gly-Pro-Arg-Arg-Phe48 (human AChE). The MAbs also reacted with the prolinerich
sequences Pro78-Gly-Phe-Glu-Gly-Thr-Glu84 and Pro88-Asn-Arg-Glu-Leu-Ser-Glu-
Asp95. These results define the interaction sites involved in the AChE-laminin interaction
and suggest that the interaction plays a role in cell adhesion. Despite the in vitro demonstrations of the importance of AChE’s non-classical functions,
the AChE knockout survives. Results from this study suggest the possibility of functional
redundancy between AChE and other molecules in early development. Using these in
vitro findings that AChE is able to bind laminin-111, information on the interaction sites,
as well as results from the monoclonal antibody (MAb) epitope analysis, the idea of
redundancy was investigated. Docking and bioinformatics techniques were used to
investigate structurally similar molecules that have comparable spatiotemporal expression
patterns in the embryonic nervous system. AChE has been shown to be involved in the
pathogenesis of Alzheimer’s disease, thus molecules associated with brain function and
neurodegeneration were also investigated. Molecules with which AChE could be possibly
redundant are syndecans, glypicans, perlecan, neuroligins and the low-density lipoprotein
receptors and their variants. AChE was observed to dock with growth arrest-specific
protein 6 (Gas6) as well as apolipoprotein E3 (ApoE-3) at the same site as the laminin
interaction. The AChE interaction site was shown to resemble the apolipoprotein-binding
site on the low density lipoprotein receptor, and related molecules, including the low
density lipoprotein receptor-related molecule (LRP) and the sortilin-related receptor
(SORL1). These molecules, along with apoE, are associated with Alzheimer’s disease.
Resemblances to the triggering receptor on myeloid cells (TREM1) were also suggested;
this is interesting as AChE has been implicated in both haematopoiesis and
haematopoietic cancers. Coimmunoprecipitation results, applied to investigate alternative
ligands for AChE, confirmed the AChE-laminin interaction in neuroblastoma cells, and
also suggested the existence of other binding partners. In conclusion, characterisation of the AChE-laminin interaction sites and investigation of
structurally similar sites in other molecules suggests a role for AChE in the stabilization
of the basement membrane of developing neural cells and provides a feasible explanation
for the survival of the knockout mouse. Furthermore, the demonstrated similarity of the
AChE interaction site to sites on molecules, notably the low density lipoprotein receptor
family and SORL1 and their apolipoprotein ligands that are implicated in the pathology
of Alzheimer’s disease, as well as the possible link to haematopoietic differentiation and
cancers, warrants further investigation. / AFRIKAANSE OPSOMMING: Talle in vitro studies wys dat die ensiem asetielcholienesterase (AChE), behalwe vir sy
klassieke rol in die hidrolise van asetielcholien (ACh), ‘n aantal nie-cholinerge rolle
vertolk insluitend in sel adhesie, in die uitgroei van neurieten, in differensiering, asook in
amyloidosis. Dit is vooraf gewys dat AChE, met behulp van elektrostatiese meganismes,
in vitro met muis laminin-111 kan bind. Dit word verneem dat die area op AChE wat
herken word deur monoklonale teenliggaampies (MAbs), moontlik ‘n kritiese area is met
betrekking tot differensiasie. Dieselfde MAbs is gevind om beide die laminin-interaksie,
sowel as sel adhesie van neuroblastoma selle, te inhibeer. In hierdie projek word die
struktuur en eienskappe van die betrokke kritiese areas ondersoek deur die AChE-laminin
interaksie te gebruik as sjabloon. ‘n Gedetailleerde analise van die teenliggaam epitoop
het ook geskied. Met behulp van faag vertoon, modellering en hegting, sintetiese
peptiede, ensiem-gekoppelde immunosorbent toetse (ELISAs) en konformasie interaksie
area kartering, is die betrokke interaksie areas bestudeer. Hegting van enkel-ketting
varierende fragment (scFv) volgordes, verkry vanaf die vaag vertoon, aan AChE dui dat
die hoof herkennings motiewe die 90Arg-Glu-Leu-Ser-Glu-Asp motief, die 40Pro-Pro-
Met-Gly volgorde, en die 59Val-Val-Asp-Ala-Thr-Thr (mens) motief is. ‘n Interaksie
tussen muis AChE en die 1 G4 domein van laminin is gevind. Die interaksie betrek die
basiese structure: Val2718-Arg-Lys-Arg-Leu2722; Tyr2738-Tyr2739, Tyr2789-Ile-Lys-Arg-
Lys2793; en Val2817-Glu-Arg-Lys2820. Die betrokkenheid van die AG-73 (2719-2729) area
by hierdie interaksie is bevestig met ELISA eksperimente wat sintetiese peptiede
inkorporeer. Die AG-73 area oorvleuel die heparin interaksie area op laminin. Hegtings
eksperimente wys dat die hoof komponent van die interaksie area op AChE die suur
volgorde Arg90-Glu-Leu-Ser-Glu-Asp95 op die omega-lus is. Die interaksie betrek ook die
Pro40-Pro-Val42, Arg46 (gekoppel aan Glu94 deur ‘n sout-brug) en die heksapeptied Asp61
Ala-Thr-Thr-Phe-Gln66 motiewe. Analise van die MAb epitoop wys die hoof erkennings
area as volgorde Pro40-Pro-Met-Gly-Pro-Arg-Arg-Phe48 (mens AChE). Die MAbs blyk
ook gunstig te wees teenoor prolien-ryke volgordes soos Pro78-Gly-Phe-Glu-Gly-Thr-Glu84 en Pro88-Asn-Arg-Glu-Leu-Ser-Glu-Asp95. Die areas betrokke by die AChElaminin
interaksie is dus gedefinieer en ‘n moontlike rol vir hierdie interaksie in sel
adhesie word voorgestel. Die noodsaaklikheid van AChE se nie-klassieke funksies word bevraagteken na die
oorlewing van die AChE uitklop-muis. Resultate hier dui op die moontlikheid van
funksionele oortolligheid as verduideliking hiervan, spesifiek met betrekking tot
molekules betrokke in vroëe ontwikkeling asook in die proses van neurale agteruitgang.
Deur gebruik te maak van die in vitro demonstrasies van die AChE-laminin interaksie,
informasie verkry ten opsigte van die betrokke interaksie areas, asook resultate verkry
vanaf die monoklonale teenliggaam (MAb) epitoop analise, word die idee van
funksionele oortolligheid ondersoek. Hegtings en bioinformatika tegnieke is gebruik om
molekules met soortgelyke strukture en uitdrukkings patrone in die embrioniese
senuweestelses te ondersoek. Ko-immuno presipitasie tegnieke is gebruik om so
moontlike alternatiewe ligande vir AChE te ondersoek. Moontlike funksionele
oortolligheid van AChE met die volgende molekules is gevind: syndecan; glypican;
perlecan; neuroligin; asook die lae-digtheid lipoproteien (LDL) reseptore en hul variante.
Hegting van AChE met ’growth arrest-specific’ proteien 6 (Gas6) en die apolipoproteien
E3 (apoE3) is gedemonstreer en gevind om dieselfde area as die laminin interaksie te
betrek. Die betrokke interaksie area op AChE het ooreenstemminge met die
apolipoproteien interaksie area op die LDL reseptor asook met verwante molekules soos
die lae-digtheids lipoproteien reseptor-geassosieerde molekuul (LRP) en die sortilingeassosieerde
reseptor (SORL1). Hierdie molekules, insluitend apoE, speel beduidende
rolle in die patologie van Alzheimer se siekte. Ooreenkomste tussen AChE en die
verwekkings reseptor op myeloïde selle (TREM1) is ook voorgestel, die interaksie is van
belang siende dat AChE voorheen geassosieer is met beide haematopoiesis en
haematopoietiese kankers. Ko-immuno presipitasie resultate bevestig die AChE-laminin
interaksie en dui op die moontlike teenwoordigheid van alternatiewe ligande vir AChE in vivo. In konklusie, karakterisering van die AChE-laminin interaksie areas, gepaard met
identifisering van struktureel ooreenstemmende areas in ander molekules, dui op ‘n rol
vir AChE in die stabilisering van die basale membraan en verskaf dus ‘n geldige
verduideliking vir die oorlewing van die AChE uitklop-muis. Die ooreenstemming van
die AChE interaksie area met areas op ander molekules (spesifiek geassosieer met
Alzheimer se siekte), asook die moontlike assosiasie van AChE met haematopoietiese
differensiering en kanker, lê die grondslag vir verdere ondersoeke.
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The Purification and Identification of Interactors to Elucidate Novel Connections in the HEK 293 Cell LineHawley, Brett 23 November 2012 (has links)
The field of proteomics studies the structure and function of proteins in a large scale and high throughput manner. My work in the field of proteomics focuses on identifying interactions between proteins and discovering novel interactions. The identification of these interactions provides new information on metabolic and disease pathways and the working proteome of a cell. Cells are lysed and purified using antibody based affinity purification followed by digestion and identification using an HPLC coupled to a mass spectrometer. In my studies, I looked at the interaction networks of several AD related genes (Apolipoprotein E, Clusterin variant 1 and 2, Low-density lipoprotein receptor, Phosphatidylinositol binding clathrin assembly protein, Alpha-synuclein and Platelet-activating factor receptor) and an endosomal recycling pathway involved in cholesterol metabolism (Eps15 homology domain 1,2 and 4, Proprotein convertase subtilisin/kexin type 9 and Low-density lipoprotein receptor). Several novel and existing interactors were identified and these interactions were validated using co-immunopurification, which could be the basis for future research.
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Contribution de la déficience en lipoprotéine lipase (LPL) au profil cardiométabolique lié à l'adiponectine chez les femmesLoucif, Yacine 04 1900 (has links)
La déficience partielle en lipoprotéine lipase (LPLD) est associée à une augmentation du risque cardiométabolique chez les hommes et les femmes. L’adiponectine, le syndrome métabolique et la ménopause sont des modulateurs importants de ce risque. L’objectif de cette étude était d’évaluer la contribution de l’adiponectine au profil de risque cardiométabolique de femmes porteuses de variants dans le gène LPL connus pour être associés avec la LPLD.
L'échantillon étudié comprenait 568 femmes d'origine canadienne-française, dont 127 avec une LPLD et 441 non LPLD (contrôles). L'influence de l'adiponectine sur le risque associé à la LPLD a été évaluée en utilisant des analyses de régression multiples prenant en compte l’influence du statut ménopausique, des variables anthropométriques, du bilan lipidique, de la glycémie à jeun et du tabagisme.
Les résultats montrent que les niveaux d'adiponectine étaient significativement plus faibles dans les groupes LPLD. La contribution des valeurs faibles d’adiponectine au profil de risque cardiométabolique des sujets LPLD était indépendante du statut ménopausique et de toutes les autres covariables étudiées. Cela suggère que l'adiponectine contribue au profil de risque cardiométabolique chez les femmes porteuses d’une mutation connue pour être associée avec la LPLD. / The cardiovascular risk significantly increases after menopause. Lipoprotein lipase (LPL) is a key enzyme in the metabolism of triglyceride (TG)-rich lipoproteins which contributes to cardiometabolic homeostasis. Adiponectin is an adipocytokine which also influences the cardiometabolic status. The objective of this study was to evaluate the contribution of plasma adiponectin to the cardiometabolic status of women carrying loss-of-function LPL gene variants (LPLD). A total of 568 French Canadian women (127 LPLD and 441 controls) were included. The association of plasma adiponectin with LPLD was assessed using multiple regression models. Cardiometabolic covariates included anthropometrics, lipids (TG, HDL-C, LDL-C, apo B), fasting glucose and smoking. Mean plasma adiponectin concentration was significantly lower in women with LPLD. Women carrying loss-of function LPL gene mutations also presented a significantly higher risk of coronary artery disease. In conclusion, these results suggest that low plasma adiponectin significantly contributes to the cardiometabolic risk profile of postmenopausal women carrying loss-of-function LPL gene mutations, independently of anthropometrics, lipids and other covariates.
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Einfluss von körperlichem Training bei chronischer Herzinsuffizienz auf die Transkription von proangiogenen microRNAs in EndothelzellenRiedel, Saskia 01 February 2017 (has links) (PDF)
Die chronische Herzinsuffizienz ist ein schwerwiegendes progredientes Krankheitsbild, das sich neben Dyspnoe und abnehmender Leistungsfähigkeit in einer nachgewiesenen Verschlechterung der HDL-Funktion manifestiert. In zahlreichen Studien, in denen der Einfluss von körperlichem Training auf die Progredienz der chronischen Herzinsuffizienz untersucht wurde, korrelierte dauerhaftes Ausdauertraining mit einer Verbesserung der eNOS-Aktivität und damit der HDLFunktion in Gefäßen. Ein Regulationsmechanismus von Endothelzellen besteht in der Expression von angiogenen microRNAs, die über negative Regulation die Proteinexpression beeinflussen. Ziel dieser Studie ist es nun, einen möglichen Zusammenhang zwischen der HDL-Funktionalität und der microRNA-Expression in Endothelzellen zu prüfen und damit die Funktionsänderung von HDL bei Herzinsuffizienten auf molekularer Ebene nachzuweisen. Zudem soll eine Beeinflussung der HDL-Funktion durch körperliches Training geprüft werden. Dafür wurde das HDL von gesunden und herzinsuffizienten Probanden (NYHAIII-Stadium) vor und nach einem vier- bzw. zwölfwöchigen Trainingsprogramm aus dem Plasma isoliert. Anschließend erfolgte mit dem gewonnenen HDL die 24-stündige Inkubation von HAEC-Kulturen. Nach Isolation der microRNAs aus dem gewonnenen Zelllysat konnte die Menge ausgewählter proangiogener miRs über RT-PCR quantifiziert werden. Die molekularbiologische Analyse der Proben zeigte eine, im Vergleich zu den Kontrollzellen, signifikant verringerte Menge an miR-21, -126 und -222 in den, mit HDLNYHAIII-inkubierten, Endothelzellen. Die miR-Expression der Endothelzellen zeigte nach dem Trainingsprogramm eine Annäherung an das Expressionsniveau der Kontrollen. Aus der dargelegten Studie wird so ersichtlich, dass das HDL von Herzinsuffizienten die Expression von proangiogenen microRNAs in Endothelzellen hemmt, was scheinbar in Korrelation mit der Ausbildung von endothelialen Dysfunktionen bei Herzinsuffizienz steht. Zudem konnte gezeigt werden, dass körperliches Training mit einer verbesserten Endothelfunktion über die Erhöhung der miR-Expression in Endothelzellen einhergeht.
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Structural studies of HDL and applications of EM on membrane proteinsZhu, Lin January 2017 (has links)
A large number of proteins interact with biological membranes, either integrated in the membrane (PepTSo2), embedded on a membrane surface (5-lipoxygenase) or encircling a cutout of lipid bilayer (apolipoprotein1 (apoA-I). They function as transporters, receptors or biocatalysts in cellular processes like inflammation or cholesterol transport which are touched upon here. Malfunction of specific membrane proteins are the cause for several diseases or disorders. Knowledge of protein structure supports understanding of its mechanism of function. Here, transmission electron microscopy (TEM) was used for structure determination. To obtain structure information to high resolution for membrane proteins, normally surrounded by lipids, demands specific methods and materials for stabilization. Stabilized in detergent the structure of the bacterial transporter PepTSo2 was shown to form a tetramer even bound to substrate. However, with a protein based stabilizer, Salipro, the structure of PepTSo2 could be determined to high resolution. High density lipoprotein (HDL) in blood plasma, involved in the removal of cholesterol from peripheral tissues, have a central role in cardiovascular function, metabolic syndrome and diabetes. The HDL-particle is composed of two copies of ApoA1 and around hundred lipid molecules. From TEM data, for the first time the clearly discoidal shape could be shown by 3-dimendional reconstructions. These were used for modelling the ApoA1 protein dimer by a "biased fitting" procedure. The results indicate how ApoA1 folds around a lipid bilayer in a disc-shaped structure. Modified HDL called nanodiscs were here used to show the Ca2+ dependent binding of 5-lipoxygenase on the nanodisc bilayer and thereby increased production of the inflammatory mediator leukotrieneA4. Dimerization of 5-lipoxygenase inactivates these functions. / <p>QC 20170323</p>
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