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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.
1

Ferroportin: Mechanisms of Iron Transport and Regulation by Hepcidin

Ruwe, Theodore January 2021 (has links)
No description available.
2

Electrophysiological Studies on Escherichia coli Protein-conducting Channel

Lin, Bor-Ruei 03 December 2008 (has links)
We have developed a novel, sensitive and less time-consuming method to detect activity of the SecA-dependent protein-conducting channels. Nanogram levels of E. coli inverted membrane vesicles were injected into Xenopus oocytes, and ionic currents were recorded using the two-electrode voltage clamp. Currents were observed only in the presence of E. coli SecA in conjunction with E. coli membranes. The observed currents showed outward rectification in the presence of KCl as permeable ions and were significantly enhanced by coinjection with the precursor protein, proOmpA, or active LamB signal peptide. Channel activity was blockable with sodium azide or adenylyl 5’-(β, γ-methylene)-diphosphonate, a non-hydrolyzable ATP analog, both of which are known to inhibit SecA protein activity. Channel activity was also stimulated by oocyte endogenous precursor proteins, which could be inhibited by puromycin. In the presence of puromycin, exogenous proOmpA or LamB signal peptides, but not defective signal peptides, stimulated the ionic currents. We also measured SecA-dependent currents with membranes depleted of SecYEG. Wild-type LamB signal peptides, or precursor proteins stimulated ionic currents following a co-injection of SecYEG¯ membranes with puromycin. Excess exogenous SecA stimulated ionic currents through SecYEG¯ membranes. Similar activities of added SecA were observed with reconstituted membranes depleted of SecYEG. Currents through such SecYEG-depleted membranes were also stimulated by addition of defective LamB signal peptides and unfolded mature PhoA protein. In contrast, currents produced by the membranes containing wild-type SecYEG were not so stimulated, but ionic currents were stimulated through mutant strains, similar to PrlA (SecY) suppressors, e.g. PrlA4, or PrlA665 membranes, suggesting that the proofreading function of SecY was bypassed in these membranes. We have observed that azide can inhibit ionic currents when E. coli wild-type MC4100 membranes were injected with proOmpA or LamB signal peptides into Xenopus oocytes. However, such inhibition was lost when observed with oocyte-endogenous signal peptides in the absence of bacterial signal peptides. Moreover, azide did not show complete inhibition upon using SecYEG¯ membranes or SecYEG¯ reconstituted membranes plus excess SecA in the presence or absence of LamB signal peptides. Such conformational alterations reflect different sensitivity in response to azide during the opening of protein-conducting channels.
3

Cholesterol Oxidase Modified Microelectrodes for Detection of Cholesterol in the Plasma Membrane of Single Cells

Devadoss, Anando January 2006 (has links)
No description available.
4

Etude des protéines à motif PQ : Identification d'un nouveau transporteur lysosomal impliqué dans le traitement de la cystinose et analyse bioinformatique de la famille protéique / PQ-loop Protein Study : Identification of a New Lysosomal Transporter Involved in Cystinosis Treatment and Bioinformatic Analysis of its Proteic Family

Jézégou, Adrien 25 November 2014 (has links)
Le transport de composés à travers les membranes biologiques est crucial pour la physiologie des cellules eucaryotes. Cependant la fonction de nombreux transporteurs putatifs reste inconnue. C’est notamment le cas de nombreux transporteurs intracellulaires exportant les catabolites du lysosome. Le transporteur lysosomal de cystine, baptisé cystinosine, se caractérise par la présence d’un motif dupliqué appelé " boucle PQ ". Sa dysfonction entraîne une maladie lysosomale, la cystinose, caractérisée par l'accumulation de cystine dans les lysosomes. Les protéines possédant un motif PQ sont retrouvées plus souvent dans les cellules eucaryotes et, à l'exception de la cystinosine, leur fonction reste inconnue. Dans cette thèse, nous démontrons qu'une autre protéine à motif PQ, PQLC2 est le transporteur responsable de l'efflux lysosomal des acides aminés cationiques et qu'il est impliqué dans le traitement de la cystinose.L'hypothèse de départ était basée, d'une part, par sur des prédictions par analyse protéomique de la localisation lysosomale de PQLC2 et, d'autre part, sur des résultats chez S.cerevisiae impliquant les orthologues putatifs de PQLC2, situés à la membrane de la vacuole, dans l'homéostasie des acides aminés cationiques. En utilisant une approche consistant à délocaliser PQLC2 à la membrane plasmique et à acidifier le pH extracellulaire pour mimer la lumière acide du lysosome, nous avons pu, par mesure d'accumulation intracellulaire de composés radiomarqués et par mesure électrophysiologique sur cellule entière, faire la preuve du transport sélectif, actif à bas pH et de faible affinité des acides aminés cationiques par PQLC2. Dans une seconde partie, nous avons mis en évidence l'implication de ce transporteur dans l'efflux lysosomal du produit de réaction entre la cystine accumulée dans les lysosomes de cellules de patients cystinotiques et le principe actif (cystéamine) du traitement pharmacologique de la cystinose.Enfin, dans une dernière partie, nous avons effectué une analyse bioinformatique préliminaire des protéines à motif PQ qui exploitait la pseudo-symétrie de ces protéines pour identifier des résidus potentiellement impliqués dans l'activité de transport. / Transport of solutes across biological membranes is crucial to eukaryotic cell physiology. However, the function of many putative transporters remains unknown, such as the proteins responsible for lysosomal export of metabolites. Cystinosin, the lysosomal cystine exporter defective in cystinosis, is characterized by a duplicated motif termed the PQ loop. PQ-loop proteins are more frequent in eukaryotes than in prokaryotes, and, except for cystinosin, their molecular function remains unknown. Here we show that another PQ-loop protein, PQLC2, is a lysosomal transporter for cationic amino acids and that it is required for the treatment of cystinosis. The hypothesis that PQLC2 is a lysosomal metabolite transporter was based on a proteomic study predicting that PQLC2 is located at the lysosomal membrane and on a genetic study that linked putative yeast orthologues with cationic amino acid homeostasis. Using an approach that consisted in misrouting PQLC2 to the plasma membrane of frog oocytes and in acidifying the extracellular medium to mimic the acidic lysosomal lumen, we showed an accumulation of radiolabelled cationic amino acids into mRNA-injected oocytes and an electrogenic, inward current due to a selective, pH-dependent, low-affinity transport of cationic amino acids by PQLC2. Moreoever, we showed that PQLC2 exports a key chemical intermediate (cysteamine-cysteine mixed disulfide) from cystinotic lysosomes treated with the aminothiol drug cysteamine, thus explaining the mechanism underlying the current drug therapy of cystinosis. Finally, in a last chapter, we performed a preliminary bioinformatic study of the family of PQ-loop proteins that took advantage of the pseudo-symmetric structure of these proteins to identify residues potentially important for the transport activity.

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