Global ETD Search

51	N-Unsubstituted Glucosamine Residues in Heparan Sulfate and Their Potential Relation to Alzheimer's Disease Westling, Camilla January 2003 (has links) Heparan sulfate (HS) is a linear polysaccharide, located on the surface and in the extracellular matrix of most cells, that regulates functions of numerous proteins. HS-protein interaction is mainly mediated by sulfate groups found in N-sulfated (NS) regions of the HS, but may also involve rare HS substituents such as N-unsubstituted glucosamine (GlcNH2) residues. The location of GlcNH2 in an HS-epitope recognized by the monoclonal antibody 10E4, that specifically stains the prion lesions in scrapie-infected murine brain, suggests an involvement of GlcNH2 in prion disease and other amyloid-related disorders. HS in general is strongly associated with amyloidosis, including Alzheimer’s disease (AD). Therefore, the aims of this thesis were to structurally characterize GlcNH2-containing HS sequences found in native tissues, to further study HS epitopes recognized by 10E4, and to investigate the possible role(s) of GlcNH2 and other HS structures in binding to amyloid β peptide (Aβ) (core material in AD plaque lesions, also stained by 10E4). The GlcNH2 content (0.7-4% of total disaccharide units) varied between HS from different tissues. Most GlcNH2 units were found in poorly modified N-acetylated (NA-) or NA/NS-domains, located toward the polysaccharide-protein linkage region. Binding of human cerebral cortex HS to Aβ(1–40) monomers requires N-, 2- and 6-O-sulfation of HS, while binding to Aβ fibrils requires N- and 2-O-sulfation only. GlcNH2 units do not appreciably contribute to interaction with Aβ. Aβ fibril-binding HS domains also bind to fibroblast growth factor 2 (FGF-2), indicating that Aβ (neurotoxic) and FGF-2 (neuroprotective) may compete for common binding sites in HS. However, Aβ had no effect on FGF-2-induced MAPK signaling in NIH 3T3 fibroblasts. Continued studies on 10E4-antigenic HS epitope(s) showed that binding of 10E4 to the previously identified antigenic tetrasaccharide, ∆UA-GlcNH2-GlcA-GlcNAc, requires the nonreducing hexuronic acid (∆UA) to be 4,5 unsaturated (induced by lyase cleavage), and thus is artificial. Further studies are needed to clarify the potential involvement of GlcNH2 in 10E4-recognition of the native HS epitope(s). Biochemistry heparan sulfate N-unsubstituted glucosamine Alzheimer's disease amyloid beta peptide amyloidosis 10E4 antibody fibroblast growth factor 2 Biokemi Biochemistry Biokemi
52	Symbiose mycorhizienne : développement de nouvelles méthodes pour la synthèse de glycoconjugues bioactifs Stevenin, Arnaud 23 September 2011 (has links) (PDF) Les symbioses bactérie-légumineuse (nodulation) et champignon-plante (mycorhization) présentent un intérêt agrobiologique et écologique majeur ; elles permettent aux plantes de croître naturellement sur un sol aride et peu fertile. Il a été démontré très récemment que les signaux impliqués dans la mise en place de la symbiose endomycorhizienne à arbuscule (facteurs "Myc") sont très proches de ceux de la nodulation. Il s'agit de molécules appartenant à la famille des lipo-chitooligosaccharides. Afin de réaliser la synthèse de ces molécules, deux nouvelles méthodologies ont été développées. L'ouverture oxydante d'acétals de 4,6-O-benzylidène de plusieurs glycopyranosides (en série gluco, galacto et manno) par le diméthyldioxirane (DMDO) a été étudiée. Le contrôle de la régiosélectivité a été effectué grâce au groupement protecteur introduit sur la fonction alcool de la position 3. La formation directe de β-glycosides de la N-acétyl-D-glucosamine par catalyse au triflate de fer (III) a été étudiée. La réaction a été menée sous irradiation micro-ondes ou en flux continu (système minifluidique Vapourtec®). Une nouvelle stratégie pour la synthèse du facteur [Myc-IV (C16:0, S)] a ensuite été établie. Nous avons utilisé un réactif peu toxique et non odorant pour introduire le motif thio nécessaire à la formation de deux liaisons glycosidiques. Le disaccharide précurseur de l'unité réductrice a été obtenu grâce à la première méthodologie développée au cours de cette thèse. [CHIM:OTHE] Chemical Sciences/Other Symbiose mycorhizienne Glycoconjugés bioactifs Acétals de 4 6-O-benzylidène Diméthyldioxirane Régiosélectivité N-acétyl-D-glucosamine Triflate de fer (III) Facteur Myc Lipo-chitooligosaccharide Thiol non odorant
53	Production of neocartilage tissues using primary chondrocytes / Fabrikation av konstgjord brosk med primära broskceller Ylärinne, Janne January 2016 (has links) Hyaline cartilage is a highly specialized tissue, which plays an important role in the articulating joints of an individual. It provides the joints with a nearly frictionless, impact resisting surface to protect the ends of the articulating bones. Articular cartilage has a poor self-repair capacity and, therefore, it rarely heals back to normal after an injury. Overweight, injuries, overloading and genetic factors may initiate a degenerative disease of the joint called osteoarthritis. Osteoarthiritis is a major global public health issue. Currently, the most used treatment for large articular cartilage defects is joint replacement surgery. However, possibilities to replace this highly invasive operation with strategies based on tissue engineering are currently investigated. The idea of the tissue engineering is to optimize the use of the cells, biomaterials and culture conditions to regenerate a new functional tissue for the defect site. The goal of this thesis was to manufacture cartilage tissue in cell culture conditions in vitro. Bovine primary chondrocytes isolated from the femoral condyles were used in all the experiments for neocartilage production. The samples were collected for histology, gene expression level quantifications, and analyses of proteoglycan (PG) content and quality. The histological sections were stained for type II collagen and PGs, the quantitative RT-PCR was used to observe the relative expressions of aggrecan, Sox9, procollagen α2(I) and procollagen α1(II) genes. The PGs were quantified using a spectrophotometric method, and agarose gel electrophoresis was used to separate the PGs according to their size. In the two first studies, we optimized the culture conditions of in vitro scaffold-free culture technique to produce the native-type hyaline cartilage of a good quality. We found out that high glucose concentration and hypertonic medium at 20% oxygen tension promoted the best hyaline-like neocartilage tissue production. Glucosamine sulfate supplementation, low oxygen tension, 5 mM glucose concentration and a transient TGF-β3 supplementation were not beneficial for the neocartilage formation in the scaffold-free cell culture system. In the third study, we used these newly defined, optimized culture conditions to produce the neocartilage tissues in the HyStem™ and the HydroMatrix™ scaffold materials and we compared these tissues to the ones grown as scaffold-free control cultures. We noticed that there was no difference between the controls and the scaffolds, and occasionally the scaffold-free controls had produced better quality cartilage than the ones with the scaffolds. Overall, the neocartilage tissues were of good hyaline-like quality in the third study. Their extracellular matrix contents were close to the native cartilage, although the neotissues lacked the zonal organization typical to the normal articular cartilage. The tissues had the right components, but their ultrastructure differed from the native cartilage. In conclusion, we were able to optimize our in vitro neocartilage culture method further, and discovered a good combination of the culture conditions to produce hyaline-like cartilage of good quality. Surprisingly, the scaffold materials were not beneficial for the cartilage formation. / Lasi- eli hyaliinirusto on pitkälle erikoistunutta kudosta, jolla on erittäin tärkeä rooli yksilön nivelten toiminnassa. Kudos suojaa ruston alapuolista luuta muodostamalla lähes kitkattoman ja joustavan liikkumista helpottavan pinnan. Lasiruston oma uusiutumiskyky on hyvin heikko, ja näin ollen kudos vain harvoin paranee alkuperäisen kaltaiseksi vaurion jälkeen. Ylipaino, vammat, liiallinen kuormitus tai geneettiset tekijät voivat käynnistää rustokudoksen rappeutumisen. Tätä tilaa kutsutaan nivelrikoksi. Nivelrikko on valtava kansanterveydellinen ongelma. Keinonivelleikkaus on nykyisellään ainoa hoitokeino pinta-alaltaan laajojen nivelruston vaurioiden hoitoon. Vaihtoehtoja tämän suuren ja invasiivisen kirurgisen operaation korvaamiseksi tutkitaan kuitenkin koko ajan ympäri maailmaa. Kudosteknologian ajatuksena on optimoida solujen, biomateriaalien ja erilaisten kasvatusolosuhteiden käyttö uuden, alkuperäisen kaltaisen toiminnallisen kudoksen luomiseksi vauriokohtaan. Väitöskirjan kaikissa kolmessa osatutkimuksessa uudisrustokudoksia tuotettiin käyttäen naudan polven rustosta eristettyjä primäärisiä rustosoluja. Näytteet kerättiin histologisia analyysejä, geenin ilmentymistutkimuksia ja proteoglykaanisisällön ja -jakauman (PG) analyyseja varten. Histologisista leikkeistä värjättiin tyypin II kollageeni ja PG:t, ja kvantitatiivista RT-PCR -menetelmää käytettiin aggrekaani-, Sox9-, prokollageeni α2(I)- ja prokollageeni α1(II)-geenien suhteellisten ilmentymistasojen määrittämiseen. Proteoglykaanisisältö analysoitiin käyttäen spektrofotometristä menetelmää, ja PG:t eroteltiin kokonsa perusteella agaroosigeelielektroforeesia käyttäen. Kahdessa ensimmäisessä osatutkimuksessa optimoitiin tukirakenteetta kasvattujen uudisrustojen kasvatusolosuhteita natiivin kaltaisen lasiruston tuottamiseksi. Havaitsimme, että korkea glukoosipitoisuus ja hypertoninen elatusaine yhdistettynä 20 % happiosapaineeseen tuotti parhaimman laatuista uudisrustokudosta tutkituista yhdistelmistä. Glukosamiinisulfaatin lisäys, matala happiosapaine, 5 mM glukoosi konsentraatio tai TGF-β3:n lisääminen alkuvaiheessa eivät edesauttaneet uudisrustokudosten muodostumisessa. Kolmannessa osatutkimuksessa otettiin käyttöön uudet, hyväksi havaitut kasvatusolosuhteet yhdistettynä HyStem™ and HydroMatrix™ -tukimateriaaleihin, ja niitä verrattiin tukirakenteettomaan kasvatusmenetelmään. Tutkimuksessa havaittiin, ettei tukirakenteettoman kontrollin tai tukimateriaalien välillä ollut mitään eroa, ja että kontrollikasvatukset tuottivat ajoittain jopa parempaa rustoa kuin tukimateriaalein kasvatetut. Kaiken kaikkiaan kaikki tuotetut uudiskudokset muistuttivat laadullisesti lasiruston kaltaista kudosta. Molekyylisisältö lähenteli natiivia rustoa, vaikkakin uudiskudoksista puuttui normaalille nivelrustolle tyypillinen vyöhykkeinen järjestäytyminen. Kudoksissa oli parhaimmillaan oikea määrä oikeita komponentteja, mutta ne eivät vain olleet järjestäytyneet oikealla tavalla. Onnistuimme optimoimaan uudisrustokudosten kasvatusmenetelmäämme. Löysimme hyvän kasvatusolosuhteiden yhdistelmän, jonka avulla kykenimme tuottamaan lasiruston kaltaista uudisrustokudosta. Hivenen yllättäenkin, tukimateriaalit eivät olleet avuksi tutkimuksessamme uudisrustokudoksia muodostettaessa. primary chondrocytes articular cartilage tissue engineering neocartilage scaffold scaffold-free hyaluronan self-assembling peptide TGF-β3 glucosamine sulfate hypoxia hypertonic medium glucose
54	Determinação da estrutura cristalográfica da enzima da Glucosamina-6-fosfato desaminase de E.coli K12 e seus complexos com ativador alostérico e inibidor / Crystal structure of enzyme glucosamine-6-phosphate deaminase de E. coli K12 and its complexes with allosteric activator and inhibitor Marcos Roberto de Mattos Fontes 07 August 1995 (has links) A enzima Glucosamina-6-fosfato desaminase (GlcN6P desaminase) é envolvida na conversão reversível da D-glucosamina-6-fosfato (GlcN6P) em Fru6P e amônia, como parte do caminho metabólico de aminoaçúcares como fonte de energia celular. A enzima hexamérica (peso mol. 178200) exibe uma cooperatividade homotrópica intensa em direção à GlcN6P a qual é modulada alostericamente pelo ativador N-acetil-D-glucosamina 6-fosfato (GlcNAc6P). A GlcN6P desaminase foi cristalizada no grupo espacial R32, com parâmetros de rede a = b = 125.9 &#197 e c = 223.2 &#197 e um conjunto de dados à 2.1 &#197 de resolução foi coletado usando radiação de luz síncrotron (Horjales et ai., 1992). A procura no banco de dados de seqüências OWL não mostrou homologia significante com qualquer outra família de proteína, desta maneira a determinação da estrutura foi feita pela técnica de substituição isomórfica múltipla (MIR) a partir de dois derivados, um composto de platina, o K2PtCl4 e um complexo de mercúrio, o ácido mersálico. O mapa MIR a 3 &#197 de resolução mostrou contornos claros e utilizando técnicas de nivelamento de solvente (solvent flattening) estendeu-se as fases até 2.5 &#197. A enzima cristaliza-se com dois monômeros na unidade assimétrica. A densidade eletrônica final foi interpretada com o auxílio do programa gráfico \'O\', sendo possível determinar sem ambigüidade 230 dos 266 resíduos de cada monômero; a partir daí foram usados subseqüentes mapas de Fourier diferença para a localização de todos os outros resíduos. O refinamento do modelo foi feito utilizando o programa X-PLOR (Brünger, 1993), usando a rotina simulated annealing, obtendo o fator R final de 17.4% com 348 moléculas de água e quatro íons inorgânicos de fosfato. O enovelamento do monômero tem uma estrutura do tipo &#945/&#946 com uma folha-&#946 pregueada paralela central com sete fitas com topologia 4x, 1x, 1x, -3x, -1x, -1x, envolvida por ambos os lados por oito hélices-&#945 e uma hélice 310 com duas voltas. A sexta fita da folha-&#946 central tem um prolongamento no C-terminal que faz parte de uma segunda folha-&#946 antiparalela de três fitas com topologia 2, -1. O hexâmero tem uma simetria local 32, com dois trímeros empacotados frente-a-frente com uma rotação relativa de 15&#176 em tomo do eixo de ordem 3 e ligados por pontes salinas e algumas interações hidrofóbicas em tomo do eixo não cristalográfico de ordem 2. As moléculas de cada trímero formam um contato não usual de três resíduos Cis 219 próximo ao eixo de ordem três. Os complexos com ativador alostérico (GlcNAc6P) e inibidor competitivo (2-desoxi 2-amino glucitol 6-fosfato) foram co-cristalizados isomorficamente com a estrutura nativa. Os mapas Fourier diferença mostram claramente densidades para os ligantes, definindo sem ambigüidade o sítio ativo e alostérico. O refinamento dos complexos produziu a mesma conformação da proteína nativa, na margem de erro experimental. Os sítios alostéricos (seis) estão localizados na interface adjacente dos monômeros de cada trímero e os sítios ativos (ou catalíticos) no lado externo de cada monômero, no C-terminal da folha-&#946 central. O monômero tem uma topologia com enovelamento similar a um domínio de ligação de NAD, excluindo os segmentos de aminoácidos 1-35, 145-188 e 243-266. As estruturas dos complexos e da nativa estão em um estado alostérico R em concordância com o modelo MWC para um sistema do tipo K (Monod et al, 1965). Um mecanismo alostérico similar ao da GlcN6P desaminase é encontrado na enzima fosfofrutoquinase (Evans, 1981). Um mecanismo catalítico é proposto para a reação de isomerisação-desaminação da enzima GlcN6P desaminase a partir do mecanismo geral para aldose-cetona isomerases. / The enzyme Glucosamine-6-phosphate deaminase (GlcN6P deaminase) is involved in the reversible conversion of D-glucosamine-6-phosphate (GlcN6P) into Fru6P and ammonia. The hexameric enzyme (mol.wt.=178200) exhibits an intense homotropic co-operativity towards GlcN6P which is allosterically modulated by the activator N-acetyl-D-glucosamine 6-phosphate (GlcNAc6P). The GlcN6P deaminase was crystallized in space group R32, with cell parameters a=b= 125.9 &#197 and c = 223.2 &#197 and a native dataset was collected to 2.1 &#197 resolution at a synchrotron source (Horjales et al, 1992). A search of the OWL sequences database has shown no significant homology with any other known protein family. Therefore, the structure determination will have to be achieved through the Multiple Isomorphous Replacement technique from two isomorphous derivatives, a platinum compound K2PtCl4 and a mercury complex, mersalyl acid. The MIR map at 3 &#197 resolution showed clear molecular boundaries and solvent flattening techniques (Wang, 1985) were used to extend the phase set to 2.5 &#197. The final electron density map was interpreted with the aid of the graphic program \'O\'. The enzyme crystallizes with a dimmer in the asymmetric unit and 230 out of the total 266 residues of each crystallographically independent monomer could be unambiguously identified in the map. The remaining residues were located after subsequent difference Fourier maps. The refinement was made with program X-PLOR (Brunger, 1993), using the simulated annealing routine, obtained R=17.4 % with 348 water molecules and four inorganic phosphate ions. The monomer fold shows an &#945/&#946 structure with a central 7-stranded &#946-sheet with topology 4x, 1x, 1x, -3x, -1x, -1x, surrounded on both sides by eight &#945-helices and 2-turn 310 -helix. The sixth strand of the central &#946-sheet is common to a second 3-stranded anti-parallel &#946-sheet with topology 2, -1. The hexamer has local 32 symmetry, with two trimmers packed in a face-to-face arrangement with a relative rotation of 15&#176 around the 3-fold axis, and linked together by salt-bridge and some hydrophobic contacts. The molecules of each trimmer have extensive contacts and show an unusual feature of the three Cys219 residues closely clustered around the 3-fold axis. The complexes with allosteric activator (GlcNAc6P) and inhibitor (2-deoxy-2-amino glucitol 6-phosphate) were co-crystallized isomorphously with the native structure. The difference Fourier maps shows clear density for the ligands, unambiguously defining the active and allosteric sites. The complexes refinement produced the same conformation of the native, within experimental error. The allosteric sites are located at the interfaces of adjacent monomers from each trimer and the active sites (or catalytic) lie at the external side of each monomer, at the C-terminal end of the central parallel &#946-sheet. The monomer has a similar folding topology as a typical NAD binding domain, excluding the segments of aminoacids 135, 145-188 and 243-266. The native and complexes structures are at the allosteric state R concerted with MWC model for a K-system (Monod et al, 1965). A similar allosteric mechanism is found in the enzyme phosphofructokinase (Evans, 1981). A catalytic mechanism is proposed for the isomerisation-deamination reaction of the enzyme from general mechanism for aldo-keto isomerases. Cristalografia Difração de raios-X Glucosamina-6-fosfato desaminase Mecanismo alostérico Mecanismo catalítico Allosteric mechanism Catalytic mechanism Crystallography Glucosamine-6-phosphate deaminase X-ray diffraction
55	Avaliação da atividade anti-inflamatória de condroitim sulfato e glucosamina em modelo experimental de colite ulcerativa em ratos Oliveira, Luiz Gustavo de 22 March 2013 (has links) Submitted by isabela.moljf@hotmail.com (isabela.moljf@hotmail.com) on 2017-05-19T13:37:35Z No. of bitstreams: 1 luizgustavodeoliveira.pdf: 3109049 bytes, checksum: 4df3b04529f2b0980313cfda47b84ab7 (MD5) / Approved for entry into archive by Adriana Oliveira (adriana.oliveira@ufjf.edu.br) on 2017-05-19T14:46:00Z (GMT) No. of bitstreams: 1 luizgustavodeoliveira.pdf: 3109049 bytes, checksum: 4df3b04529f2b0980313cfda47b84ab7 (MD5) / Made available in DSpace on 2017-05-19T14:46:00Z (GMT). No. of bitstreams: 1 luizgustavodeoliveira.pdf: 3109049 bytes, checksum: 4df3b04529f2b0980313cfda47b84ab7 (MD5) Previous issue date: 2013-03-22 / Doenças inflamatórias intestinais, entre elas colite ulcerativa e doença de Crohn, compreendem um amplo espectro de afecções que apresentam em comum inflamação crônica do trato gastrointestinal. Colite ulcerativa afeta exclusivamente o cólon e o reto, possui etiologia ainda pouco conhecida podendo estar relacionada com fatores ambientais, genéticos e de resposta imune. O tratamento se baseia em medicamentos como aminossalicilatos, glicocorticóides e imunossupressores, porém seus efeitos colaterais atrapalham a adesão do paciente ao tratamento por longos períodos. Condroitim sulfato (CS) e glucosamina (GlcN) são atualmente indicados para o tratamento de doenças inflamatórias, como a osteoartrite, principalmente por apresentarem efeito anti-inflamatório ao diminuírem a ação do fator de transcrição NF-kB diminuindo a expressão de metaloproteases (MMP), TNF-α, iNOS entre outros mediadores inflamatórios. O objetivo deste trabalho foi analisar os efeitos da associação de CS e GlcN na colite ulcerativa experimental induzida por dextran sulfato de sódio (DSS) em ratos Wistar. Para isso foram avaliados o índice de atividade da doença (IAD), parâmetros hematológicos e bioquímicos, morfológicos e a atividade de MMP-2 e -9 da matriz extracelular no intestino grosso, concentração de NO tecidual e concentração de glicosaminoglicanos. Os animais foram divididos em quatro grupos: (1) controle, (2) controle + CS/GlcN, (3) DSS , (4) DSS + CS/GlcN. Observamos que o tratamento com CS/GlcN melhorou a severidade da colite aguda em ratos, verificado pela redução do score histológico e melhora de parâmetros hematológicos. CS/GlcN também reduziu a destruição de células caliciformes observados pelo azul de alcian, bem como a produção de óxido nítrico, a atividade de mieloperoxidase e metaloproteases, principalmente de MMP-9. Além disso, foi observado uma redução na concentração de GAGs total no grupo DSS + CS/GlcN quando comparado ao grupo DSS. Portanto, a administração de CS/GlcN apresentou melhoras em alguns dos parâmetros avaliados principalmente na atividade de MMP-9, mostrando um potencial destes compostos para futura utilização no tratamento dessa patologia. / Inflammatory bowel disease, including ulcerative colitis and Crohn's disease comprising a broad spectrum of diseases those have in common chronic inflammation of the gastrointestinal tract. Ulcerative colitis affects only the colon and rectum, has still poorly understood etiology and this could may be related to environmental factors, genetic and immune response. Treatment is based on drugs as aminosalicylates, immunosuppressants and glucocorticoids, but its side effects hinder patient compliance with treatment for long periods. Chondroitin sulphate (CS) and glucosamine (GlcN) are currently indicated for treatment of inflammatory diseases such as osteoarthritis, mainly because of the anti-inflammatory effect by decreasing the activity of transcription factor NF-kB and decreasing the expression of metalloproteases (MMP), TNF-α, iNOS and other inflammatory mediators. The objective of this study was to analyze the effects of the combination of CS and GlcN in experimental ulcerative colitis model induced by dextran sulfate sodium (DSS) in rats. To do so we evaluated the disease activity index (DAI), haematological and biochemical parameters, morphological changes and activity of MMP-2 and -9, NO and glycosaminoglycans concentration in the large intestine. Animals were divided into four groups: (1) control, (2) control + CS / GlcN, (3) DSS-induced colitis, (4) DSS + CS / GlcN. We observed that treatment with CS/GlcN improved the severity of acute colitis in rats verified by histological score reduction and improvement in hematological parameters. CS/GlcN also reduced goblet cells destruction observed by alcian blue, as well as nitric oxide production, the activity of myeloperoxidase and metalloproteases, especially MMP-9. Moreover, we observed a reduction in the concentration of total GAG + DSS group CS / GlcN when compared to DSS. Therefore, administration of CS/GlcN showed improvements in some of the parameters evaluated mainly on the activity of MMP-9, showing a potential future use of these compounds for the treatment of this pathology. CNPQ::CIENCIAS DA SAUDE Doença inflamatória intestinal Colite ulcerativa Dextran sulfato de sódio Condroitim sulfato Glucosamina Inflammatory Bowel Disease Ulcerative colitis Dextran sodium sulfate Chondroitin sulfate Glucosamine
56	FPIN's Clinical Inquiries. Glucosamine and Chondroitin for Osteoarthritis Fox, Beth A., Schmitz, Evan D., Wallace, Richard 01 April 2006 (has links) No description available. arthralgia (drug therapy etiology) chondroitin (therapeutic use) glucosamine (therapeutic use) humans osteoarthritis (complications drug therapy) practice guidelines as topic treatment outcome
57	Ligands dérivés de saccharides et, ou supportés par un bras poly(éthylène) glycol : synthèse et applications en catalyse organométallique / Ligands derived from saccharides and, or supported on poly(ethylene) glycol arm : synthesis and applications in organometallic catalysis Adidou, Ouissam 16 October 2009 (has links) La synthèse de deux familles de ligands a été envisagée. La première famille de ligands concerne la préparation de nouveaux ligands dérivés de la D-glucosamine ou du D-glucose qui seront engagés dans la réaction de substitution allylique de type Tsuji-Trost en phase homogène. La deuxième famillede ligands concerne la préparation de ligand supportés par un bras poly(éthylène) glycol et dérivés dela D-glucosamine ou de la di-(2-pyridyl)méthylamine. Ces ligands hydrosolubles ont été engagés dans deux réactions pallado-catalysées en phase aqueuse à savoir la substitution allylique de type Tsuji-Trost et la réaction de couplage croisé de type Suzuki-Miyaura, respectivement. / Ligands derived from saccharides and, or supported on poly(ethylene) glycol arm: synthesis and applications in organometallic catalysis. The synthesis of two types of ligands has been investigated. The first family of ligands has been the preparation of new ligands derived from D-glucosamine or D-glucose, which have been tested in the allylic substitution of Tsuji-Trost in homogeneous phase. The second one has een the preparation of ligand supported on poly(ethylene) glycol arm and derived from D-glucosamine or di-(2- pyridyl)methylamine. These last hydrosoluble ligands have been tested in two Pd-catalyzed reactions in aqueous phase: the allylic substitution of Tsuji-Trost and the cross-coupling Suzuki-Miyaura reaction, respectively. D-glucosamine D-glucose Di-(2-pyridyl)méthylamine Poly(éthylène) glycol Ligands hydrosolubles D-glucosamine D-glucose Di-(2-pyridyl)methylamine Poly(ethylene) glycol Hydrosoluble ligands Allylic substitution of Tsuji-Trost Cross-coupling Suzuki-Miyaura reaction 547
58	Symbiose mycorhizienne : développement de nouvelles méthodes pour la synthèse de glycoconjugues bioactifs / Mycorrhizal symbiosis : development of new methods for synthesis of bioactive glycoconjugates Stevenin, Arnaud 23 September 2011 (has links) Les symbioses bactérie-légumineuse (nodulation) et champignon-plante (mycorhization) présentent un intérêt agrobiologique et écologique majeur ; elles permettent aux plantes de croître naturellement sur un sol aride et peu fertile. Il a été démontré très récemment que les signaux impliqués dans la mise en place de la symbiose endomycorhizienne à arbuscule (facteurs "Myc") sont très proches de ceux de la nodulation. Il s'agit de molécules appartenant à la famille des lipo-chitooligosaccharides. Afin de réaliser la synthèse de ces molécules, deux nouvelles méthodologies ont été développées. L'ouverture oxydante d'acétals de 4,6-O-benzylidène de plusieurs glycopyranosides (en série gluco, galacto et manno) par le diméthyldioxirane (DMDO) a été étudiée. Le contrôle de la régiosélectivité a été effectué grâce au groupement protecteur introduit sur la fonction alcool de la position 3. La formation directe de β-glycosides de la N-acétyl-D-glucosamine par catalyse au triflate de fer (III) a été étudiée. La réaction a été menée sous irradiation micro-ondes ou en flux continu (système minifluidique Vapourtec®). Une nouvelle stratégie pour la synthèse du facteur [Myc-IV (C16:0, S)] a ensuite été établie. Nous avons utilisé un réactif peu toxique et non odorant pour introduire le motif thio nécessaire à la formation de deux liaisons glycosidiques. Le disaccharide précurseur de l'unité réductrice a été obtenu grâce à la première méthodologie développée au cours de cette thèse. / Arbuscular mycorrhiza (AM) is a root endosymbiosis between plants and fungi. It has an agrobiological interest and a crucial ecological importance because it allows plants to grow on aride and infertile soil. Recently, the structure of the symbiotic signal "Myc factor" was identified as a mixture of lipochitooligosaccharides (LCOs). In order to propose a new synthesis of LCOs, we developed two green methodologies in glycochemistry. We performed the oxidative cleavage of 4,6-O-benzylidene acetals of various glycopyranosides (gluco, manno and galacto series) with dimethyldioxirane (DMDO) and its regioselective control with a suitable protecting group at position 3. We investigated the formation of β-glycoside of N-acetyl-D-glucosamine using catalytic iron (III) triflate. The reaction can be performed using microwave irradiation or, for scale-up synthesis, flow chemistry using Vapourtec® minifluidic system. We establish a new strategy for the total synthesis of the most abundant Myc factor [Myc-IV (C16:0, S)]. We used odorless and few toxic MbpSH reagent to introduce the activated thio residue involved in two glycosylation reactions. The disaccharide acceptor precursor of the reducing end was obtained after oxidative cleavage of the 4,6-O-benzylidene moiety by DMDO. Symbiose mycorhizienne Glycoconjugés bioactifs Acétals de 4,6-O-benzylidène Diméthyldioxirane Régiosélectivité N-acétyl-D-glucosamine Triflate de fer (III) Facteur Myc Lipo-chitooligosaccharide Thiol non odorant Mycorrhizal symbiosis Bioactive glycoconjugates 4,6-O-benzylidene acetal Dimethyldioxirane Regioselectivity N-acetyl-D-glucosamine Iron (III) triflate Myc factor Odorless thiol Lipochitooligosaccharide
59	Osteoartrite experimental em ratos: efeito de sulfato de glicosamina e sulfato de condroitina sobre a incapacitação articular e a lesão de cartilagem articular / Experimental osteoarthritis in rats: evaluation of antinociceptive and chondroprotective effects of glucosamine sulfate and chondroitin sulfate Silva Junior, Francisco Saraiva da 11 April 2007 (has links) OBJETIVOS: Avaliar o efeito de sulfato de glicosamina e sulfato de condroitina sobre a nocicepção e o dano da cartilagem articular em um modelo de osteoartrite experimental em ratos. MÉTODOS: Osteoartrite (OA) foi induzida em ratos Wistar machos por transecção do ligamento cruzado anterior (TLCA) do joelho direito. Um grupo falso-operado (SHAM) foi utilizado como controle. Animais OA foram tratados v.o. desde 7 dias antes, até o sacrifício, 70 dias após a TLCA, com sulfato de glicosamina 500 mg/kg (Glu), a combinação sulfato de glicosamina 500 mg/kg e sulfato de condroitina 400 mg/kg (GluChon), ou salina (OANT). Um grupo controle positivo recebeu meloxicam 6 mg/kg s.c. A dor articular foi avaliada pelo teste de incapacitação articular para ratos. Os animais foram sacrificados em diferentes períodos (7,14,28 e 70 dias) após a TLCA. A gravidade das lesões histopatológicas foi graduada nos fêmures após coloração por H&E e azul de toluidina através do escore da OARSI. A quantidade de glicosaminoglicanos (GAGs) extraídos da cartilagem articular dos côndilos femorais foi medida após eletroforese em gel de agarose. O tamanho molecular dos GAGs foi medido após eletroforese em gel de poliacrilamida. A liberação de NO no líquido sinovial foi medida 7 dias após TLCA. RESULTADOS: GluChon reduziu significativamente a dor articular nesse modelo (p<0,01). Glu também reduziu a dor articular, mas não se alcançou significância estatística. Os animais OA apresentaram um aumento significativo dos GAGs na cartilagem articular aos 70 dias após TLCA (77,68±3,38 µg/mg) quando comparados aos animais SHAM (53,46±4,58 µg/mg). O tamanho molecular dos GAGs foi significativamente maior nos animais OA que nos animais SHAM 70 dias após a cirurgia (p<0,01). GluChon preveniu tanto o aumento da quantidade de GAGs (54,42±5,39 µg/mg), quanto de seu tamanho molecular (p<0,05), e estes resultados acompanharam-se de melhora significativa da lesão histopatológica (p<0,05). Os resultados obtidos com Glu foram semelhantes, porém menos evidentes, e não alcançaram significância estatística. Glu aumentou significativamente a quantidade de NO na cavidade articular 7 dias após a TLCA. CONCLUSÕES: GluChon foi antinociceptivo e reduziu significativamente a incapacitação articular. A lesão da cartilagem articular no modelo de TLCA em ratos se acompanha de aumento da concentração e do tamanho molecular dos GAGs, e o tratamento com GluChon previne essas alterações e reduz o dano histopatológico. GluChon foi mais eficaz do que Glu tanto na redução da dor quanto da lesão da cartilagem articular, sugerindo benefício da combinação sobre o uso isolado de sulfato de glicosamina. / OBJECTIVES: Evaluate the antinociceptive and chondroprotective effects of glucosamine sulfate and chondroitin sulfate. METHODS: Male Wistar rats underwent anterior cruciate ligament transection (ACLT) or sham operation of the right knee. Animals were treated p.o. with glucosamine sulfate (Glu) 500 mg/kg, the combination of glucosamine sulfate 500 mg/kg and chondroitin sulfate 400 mg/kg (GluChon), or saline, since 7 days prior to surgery until the sacrifice 70 days after ACLT. A positive control group received meloxicam 6 mg/kg s.c. for antinociceptive evaluation comparisons. Joint pain was evaluated with rat incapacitation test. Animals were sacrificed 7,14,28 or 70 days after ACLT. The severity of histopathologic lesions was evaluated on femoral condyles after hematoxylin-eosin or toluidine blue staining with OARSI grading and staging system. Cartilage extracted glycosaminoglycans (GAGs) concentration was assessed after agarose gel electrophoresis. GAGs\' molecular weight was evaluated after polyacrylamide gel electrophoresis. NO release in synovial fluids was assessed 7 days after ACLT. RESULTS: GluChon reduced joint pain (p<0.01). Glu also reduced joint pain, but results did not reach statistical significance. A significant increase in articular cartilage\'s GAGs concentration was observed in OA animals (77.68±3.38 µg/mg) as compared to sham (53.46±4.58 µg/mg). OA animals also had significantly higher molecular weight GAGs than sham (p<0.01). GluChon prevented both GAG concentration and molecular weight elevations in OA animals, and that was associated with significant less cartilage damage assessed by histopathologic examination (p<0.05). Glu effects were less evident, and did not reach statistical significance. Glu was associated with significant higher concentrations of NO in synovial fluid. CONCLUSIONS: GluChon was antinociceptive on the ACLT model in rats. Articular cartilage damage was associated with increased amounts of GAG with higher molecular weight, and the prevention of these alterations with GluChon treatment was associated with less histopathologic damage. GluChon was more efficient than Glu for both pain and articular cartilage damage reduction, suggesting that combined treatment is better than glucosamine sulfate alone. Animal models Anterior cruciate ligament Artralgia Chondroitin sulfate Glicosaminoglicanas Glucosamina Glucosamine Glycosaminoglycans Joint pain Ligamento cruzado anterior Medição da dor Modelos animais Osteoarthritis Osteoartrite Pain evaluation Ratos Rats Sulfatos de condroitina
60	Osteoartrite experimental em ratos: efeito de sulfato de glicosamina e sulfato de condroitina sobre a incapacitação articular e a lesão de cartilagem articular / Experimental osteoarthritis in rats: evaluation of antinociceptive and chondroprotective effects of glucosamine sulfate and chondroitin sulfate Francisco Saraiva da Silva Junior 11 April 2007 (has links) OBJETIVOS: Avaliar o efeito de sulfato de glicosamina e sulfato de condroitina sobre a nocicepção e o dano da cartilagem articular em um modelo de osteoartrite experimental em ratos. MÉTODOS: Osteoartrite (OA) foi induzida em ratos Wistar machos por transecção do ligamento cruzado anterior (TLCA) do joelho direito. Um grupo falso-operado (SHAM) foi utilizado como controle. Animais OA foram tratados v.o. desde 7 dias antes, até o sacrifício, 70 dias após a TLCA, com sulfato de glicosamina 500 mg/kg (Glu), a combinação sulfato de glicosamina 500 mg/kg e sulfato de condroitina 400 mg/kg (GluChon), ou salina (OANT). Um grupo controle positivo recebeu meloxicam 6 mg/kg s.c. A dor articular foi avaliada pelo teste de incapacitação articular para ratos. Os animais foram sacrificados em diferentes períodos (7,14,28 e 70 dias) após a TLCA. A gravidade das lesões histopatológicas foi graduada nos fêmures após coloração por H&E e azul de toluidina através do escore da OARSI. A quantidade de glicosaminoglicanos (GAGs) extraídos da cartilagem articular dos côndilos femorais foi medida após eletroforese em gel de agarose. O tamanho molecular dos GAGs foi medido após eletroforese em gel de poliacrilamida. A liberação de NO no líquido sinovial foi medida 7 dias após TLCA. RESULTADOS: GluChon reduziu significativamente a dor articular nesse modelo (p<0,01). Glu também reduziu a dor articular, mas não se alcançou significância estatística. Os animais OA apresentaram um aumento significativo dos GAGs na cartilagem articular aos 70 dias após TLCA (77,68±3,38 µg/mg) quando comparados aos animais SHAM (53,46±4,58 µg/mg). O tamanho molecular dos GAGs foi significativamente maior nos animais OA que nos animais SHAM 70 dias após a cirurgia (p<0,01). GluChon preveniu tanto o aumento da quantidade de GAGs (54,42±5,39 µg/mg), quanto de seu tamanho molecular (p<0,05), e estes resultados acompanharam-se de melhora significativa da lesão histopatológica (p<0,05). Os resultados obtidos com Glu foram semelhantes, porém menos evidentes, e não alcançaram significância estatística. Glu aumentou significativamente a quantidade de NO na cavidade articular 7 dias após a TLCA. CONCLUSÕES: GluChon foi antinociceptivo e reduziu significativamente a incapacitação articular. A lesão da cartilagem articular no modelo de TLCA em ratos se acompanha de aumento da concentração e do tamanho molecular dos GAGs, e o tratamento com GluChon previne essas alterações e reduz o dano histopatológico. GluChon foi mais eficaz do que Glu tanto na redução da dor quanto da lesão da cartilagem articular, sugerindo benefício da combinação sobre o uso isolado de sulfato de glicosamina. / OBJECTIVES: Evaluate the antinociceptive and chondroprotective effects of glucosamine sulfate and chondroitin sulfate. METHODS: Male Wistar rats underwent anterior cruciate ligament transection (ACLT) or sham operation of the right knee. Animals were treated p.o. with glucosamine sulfate (Glu) 500 mg/kg, the combination of glucosamine sulfate 500 mg/kg and chondroitin sulfate 400 mg/kg (GluChon), or saline, since 7 days prior to surgery until the sacrifice 70 days after ACLT. A positive control group received meloxicam 6 mg/kg s.c. for antinociceptive evaluation comparisons. Joint pain was evaluated with rat incapacitation test. Animals were sacrificed 7,14,28 or 70 days after ACLT. The severity of histopathologic lesions was evaluated on femoral condyles after hematoxylin-eosin or toluidine blue staining with OARSI grading and staging system. Cartilage extracted glycosaminoglycans (GAGs) concentration was assessed after agarose gel electrophoresis. GAGs\' molecular weight was evaluated after polyacrylamide gel electrophoresis. NO release in synovial fluids was assessed 7 days after ACLT. RESULTS: GluChon reduced joint pain (p<0.01). Glu also reduced joint pain, but results did not reach statistical significance. A significant increase in articular cartilage\'s GAGs concentration was observed in OA animals (77.68±3.38 µg/mg) as compared to sham (53.46±4.58 µg/mg). OA animals also had significantly higher molecular weight GAGs than sham (p<0.01). GluChon prevented both GAG concentration and molecular weight elevations in OA animals, and that was associated with significant less cartilage damage assessed by histopathologic examination (p<0.05). Glu effects were less evident, and did not reach statistical significance. Glu was associated with significant higher concentrations of NO in synovial fluid. CONCLUSIONS: GluChon was antinociceptive on the ACLT model in rats. Articular cartilage damage was associated with increased amounts of GAG with higher molecular weight, and the prevention of these alterations with GluChon treatment was associated with less histopathologic damage. GluChon was more efficient than Glu for both pain and articular cartilage damage reduction, suggesting that combined treatment is better than glucosamine sulfate alone. Artralgia Glicosaminoglicanas Glucosamina Ligamento cruzado anterior Medição da dor Modelos animais Osteoartrite Ratos Sulfatos de condroitina Animal models Anterior cruciate ligament Chondroitin sulfate Glucosamine Glycosaminoglycans Joint pain Osteoarthritis Pain evaluation Rats

Search results