Global ETD Search

1	Neuron-ligand pathfinding on surfaces modified by laminin and laminin-derived peptides Leng, Ying. January 2006 (has links) Thesis (M.S.)--University of Delaware, 2006. / Principal faculty advisor: Thomas P. Beebe, Jr., Dept. of Chemistry & Biochemistry. Includes bibliographical references.
2	High resolution structural studies of membrane proteins using solid state NMR Aslimovska, Lubica January 2008 (has links) NMR crystallography is a new and developing area. Unlike solution state NMR, solid state NMR has the potential for structural studies of large, motionally restricted biological macromolecules, such as proteins in crystals which may, or may not, diffract. However, finding the best and the most useful sample form and geometry is still a major obstacle to rapid progress. Little has been reported about protein sample preparation for any class of protein for NMR crystallography, mainly since the availability of NMR labelled proteins is still not routine, especially for eukaryotic membrane proteins. The amino acid L-glutamate is the major excitatory neurotransmitter in the brain. Details of glutamate binding to any of its main brain or sensory receptors are not well resolved at the atomic level. In an effort to resolve the glutamate binding mechanism by solid state NMR methods, full-length taste and brain mGluR4 were expressed in E. coli, but proved to be toxic for the cells. The ligand-binding domains (LBD) of mGluR4, with various fusions for the periplasmic expression and with various fusions for expression in the cytoplasm therefore, were used. Solubilisation and then purification of the LBD from inclusion bodies is still under way, no crystals of mGluR4 for NMR were, therefore, grown. Initial NMR spectra of labelled 13C, 15N and 17O glutamate have been recorded to verify sensitivity requirements. Using homology modelling, a model for the truncated version of the ligand binding domain of mGluR4 has been constructed as a basis for designing solid state NMR experiments to probe the ligand binding site in the receptor. Bacteriorhodopsin is a large membrane protein and a model for G-protein coupled receptors (GPCRs). Spectra of bacteriorhodopsin produced in H. salinarium in purple membrane are reported here and compared to spectra of the protein crystallised from bicelles. Optimal conditions for producing spectra suitable for spectral assignment are reported as an initial step towards spectral resolution. Three differently labelled samples of bacteriorhodopsin were prepared to test the applicability of the various assignment strategies and the effects of deuteration on quality of solid state NMR spectra of a large, crystalline membrane protein. 572
3	Characterisation of the benzimidazole-binding site on the cytoskeletal protein tubulin / MacDonald, Louisa M. January 2003 (has links) Thesis (Ph.D.) --Murdoch University, 2003. / Thesis submitted to the Division of Veterinary and Biomedical Sciences. Includes bibliographical references (leaves 160-196).
4	The Mechanisms regulating exocytosis of the salivary glands of the soft tick, Ornithodorus savignyi Maritz-Olivier, Christine. January 2005 (has links) Thesis (Ph.D.)(Biochemistry)--University of Pretoria, 2005. / Title from opening screen (viewed March 28, 2006). Includes summary. Includes bibliographical references.
5	Effects of sodium pyrophosphate and pH on the kinetics of iron release from the N- and C-terminal binding sites of ovotransferrin / Cheuk, Man-sum. January 1988 (has links) Thesis (M. Phil.)--University of Hong Kong, 1989.
6	Folate binding protein : partial characterisation of bovine milk folate binding protein, includings its ligand binding / Jones, Marc. January 2004 (has links) (PDF) Thesis (M.Phil.) - University of Queensland, 2004. / Includes bibliographical references.
7	Computational studies of transmembrane helix insertion and association Chetwynd, Alan January 2011 (has links) Membrane proteins perform a variety of functions essential for the viability of the cell, including transport and signalling across the membrane. Most membrane proteins are formed from bundles of transmembrane helices. In this thesis molecular dynamics simulations have been used to investigate helix insertion into bilayers and helix association within bilayers. The potentials of mean force for the insertion of helices derived from the cystic ﬁbrosis transmembrane conductance regulator into lipid bilayers were calculated using coarse-grained molecular dynamics simulations. The results showed that the insertion free energy increased with helix length and bilayer hydrophobic width. The insertion free energies obtained were signiﬁcantly larger than comparable quantities obtained from translocon- mediated insertion experiments, consistent with a variety of previous studies. The implications of this observation for the interpretation of in vivo translocon-mediated insertion experiments, and the function of the translocon, are discussed. Coarse-grained and atomistic molecular dynamics simulations of the transmembrane region of the receptor tyrosine kinase EphA1 suggested that the transmembrane helix dimer was most stable when interacting via the glycine zipper motif, in agreement with a structure obtained by NMR spectroscopy. Coarse-grained simulations of the transmembrane region of EphA2 suggested that the dimer has two stable orientations, interacting via a glycine zipper or a heptad motif. Both structures showed right-handed dimers, although an NMR structure of the transmembrane region of EphA2 shows a left-handed dimer interacting via the heptad motif. Both structures obtained from coarse-grained simulations proved unstable when simulated at an atomistic level of detail. The potentials of mean force for dissociating the EphA1 and EphA2 dimers were calcu- lated using coarse-grained molecular dynamics calculations. Convergence of the detailed structure of the proﬁles was not conclusively shown, although association free energies cal- culated from the proﬁles were consistent over a variety of simulation times. The association free energies were slightly larger than experimental values obtained for comparable sys- tems, but consistent with similar computational calculations previously reported. However, direct comparisons are difﬁcult owing to the inﬂuence of environmental factors on reported association free energies. The potential of mean force proﬁles showed that the interaction via the glycine zipper motif for EphA1 was signiﬁcantly more stable than any other confor- mation. For EphA2 the potential of mean force proﬁles suggested that interaction via the glycine zipper and heptad motifs both provided stable or metastable conformations, with the interaction via the glycine zipper motif probably at least as stable as that via the heptad motif. 572.696
8	The Smad3 linker region transcriptional activity and phosphorylation-mediated regulation. Wang, Guannan. January 2008 (has links) Thesis (Ph. D.)--Rutgers University, 2008. / "Graduate Program in Biochemistry." Includes bibliographical references (p. 191-203).
9	Etude biochimique de mitoNEET humaine, protéine à centre [2Fe-2S], impliquée dans une voie de réparation des protéines Fe-S suite à un stress oxydatif / Biochemical studies of human mitoNEET, a [2Fe-2S] protein involved in a pathway dedicated to Fe-S protein repair after oxidative stress Mons, Cécile 20 November 2017 (has links) Présente chez les mammifères, mitoNEET (mNT) est une protéine à centre Fe-S ancrée à la membrane externe de la mitochondrie. Cette protéine dimérique possède un centre [2Fe-2S] par monomère lié de façon atypique à la protéine par trois cystéines et une histidine. Notre équipe a auparavant montré l’implication de mNT dans une nouvelle voie de réparation du centre [4Fe-4S] de l’Iron Regulatory Protein-1 (IRP-1), régulateur majeur de l’homéostasie du fer intracellulaire, par transfert du centre Fe-S de mNT à l’IRP-1 à réparer. Au cours de ma thèse, je me suis focalisée sur la caractérisation in vitro de la réaction de transfert de centre Fe-S de mNT vers une protéine réceptrice modèle, l’apo-ferrédoxine d’E. coli. En combinant des approches de biochimie et biophysique (réalisées en collaboration) à l’aide de protéines purifiées, cette étude a permis de démontrer que mNT agit comme un interrupteur moléculaire : lorsque son centre Fe-S est réduit, la protéine est extrêmement stable et le centre ne peut être ni perdu ni transféré; une fois oxydé, il peut alors être transféré à une protéine réceptrice. La présence d’oxygène n’affecte pas cette réaction même s’il s’agit d’un déterminant majeur de la stabilité de la protéine. De plus, la vitesse de transfert du centre est très sensible au pH, ce qui fait de mNT un senseur de pH. Ces études ont aussi montré que mNT est extrêmement résistante à H2O2 en comparaison à d’autres protéines de transfert de centre Fe-S. J’ai également étudié l’interaction d’une molécule anti-oxydante, le resvératrol-3 sulfate, avec mNT. Pour finir, je me suis intéressée à l’effet du glutathion sur mNT. Acteur majeur de la régulation de l’homéostasie rédox, le glutathion existe sous deux formes: oxydée (GSSG) et réduite (GSH). J’ai alors constaté que le GSH déstabilise fortement mNT à certains pH et peut même se lier à cette protéine. La fonction thiol du GSH et la formation de radicaux sur cette dernière sont clairement impliquées dans la déstabilisation de mNT. / Present in mammals, mitoNEET (mNT) is an Fe-S protein anchored to the outer mitochondrial membrane. This dimeric protein contains a [2Fe-2S] per monomer with an atypical ligation involving three cysteines and one histidine. Previously, our team proposed that mNT is involved in a new pathway dedicated to the reparation of the oxidatively damaged [4Fe-4S] cluster of human iron-regulatory protein-1 (IRP-1)/cytosolic aconitase, a key player of the regulation of cellular iron homeostasis. This reparation occurs via Fe-S cluster transfer from mNT to IRP-1 to repair. In the course of my thesis, I focused on the characterization of cluster transfer reaction from mNT to a model receptor protein, the E. coli apo-ferredoxin. Using purified proteins and combining biochemical approaches with biophysical ones performed in colaboration, this study showed that mNT acts as a redox switch: when the Fe-S cluster is reduced, the protein is extremely stable and it cannot be lost or transferred; when it is oxidized, it can be transferred to a receptor protein. Dioxygen does not affect this transfer reaction whereas this is a major determinant of protein stability. The transfer speed is highly sensitive to pH. Thus, mNT seems to act also as a pH sensor. Moreover, this study shows that mNT is extremely resistant to H2O2 compared to other Fe-S cluster transfer proteins. I also looked at the interaction of an antioxidant molecule, the resveratrol-3-sulfate, with mNT. Finally, I studied the effects of glutathione on mNT. Major player of the regulation of redox homeostasis, glutathione exists under two states: a reduced state (GSH) and an oxidized one (GSSG). I observed that GSH strongly destabilizes mNT at specific pHs and can even directly interact with the protein. The thiol function of GSH and the radical formation on this function are clearly involved in the mNT Fe-S destabilization. Biochimie des protéines Protéines Fe-S MitoNEET Transfert et stabilité de centre Fe-S Stabilité Glutathion Biochemistry of proteins Iron Sulfur protein MitoNEET Fe-S cluster transfer and stability Stability Glutathione
10	Structural modelling of transmembrane domains Kelm, Sebastian January 2011 (has links) Membrane proteins represent about one third of all known vertebrate proteins and over half of the current drug targets. Knowledge of their three-dimensional (3D) structure is worth millions of pounds to the pharmaceutical industry. Yet experimental structure elucidation of membrane proteins is a slow and expensive process. In the absence of experimental data, computational modelling tools can be used to close the gap between the numbers of known protein sequences and structures. However, currently available structure prediction tools were developed with globular soluble proteins in mind and perform poorly on membrane proteins. This thesis describes the development of a modelling approach able to predict accurately the structure of transmembrane domains of proteins. In this thesis we build a template-based modelling framework especially for membrane proteins, which uses membrane protein-specific information to inform the modelling process.Firstly, we develop a tool to accurately determine a given membrane protein structure's orientation within the membrane. We offer an analysis of the preferred substitution patterns within the membrane, as opposed to non-membrane environments, and how these differences influence the structures observed. This information is then used to build a set of tools that produce better sequence alignments of membrane proteins, compared to previously available methods, as well as more accurate predictions of their 3D structures. Each chapter describes one new piece of software or information and uses the tools and knowledge described in previous chapters to build up to a complete accurate model of a transmembrane domain. 572.696

Search results