• Refine Query
  • Source
  • Publication year
  • to
  • Language
  • 3
  • 1
  • 1
  • Tagged with
  • 7
  • 7
  • 4
  • 2
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 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

Genetics and biochemistry of potential virulence factors of Campylobacter

Grant, Kathleen Ann January 1998 (has links)
No description available.
2

Vliv glycinové smyčky na funkci "processing" peptidas mitochondriálního typu / Impact of the glycine-rich loop on the function of processing peptidases of the mitochondrial type

Kučera, Tomáš January 2014 (has links)
The majority of the mitochondrial proteins is synthetized on the cytosolic ribosomes in the form of the protein precursors bearing mitochondrion-targeting signal presequences. Once the protein precursor has reached the mitochondrial matrix the signal presequence is no longer necessary and is cleaved off by heterodimeric mitochondrial processing peptidase (MPP; α/β). Although the crystal structure of MPP is available, the MPP mechanism of function is still matter of discussion. An all atomic, non-restrained molecular dynamics (MD) simulation in explicit water was used to study in detail the structural features of the highly conserved glycine-rich loop (GRL) of the regulatory α-subunit of the yeast MPP. Wild-type and GRL-deleted MPP structures were studied both in the presence and absence of a substrate in the peptidase active site. Targeted MD simulations were employed to study the mechanism of substrate translocation from the GRL to the peptidase active site. We demonstrate that the natural conformational flexibility of the GRL is crucial for the substrate translocation process from outside the enzyme towards the MPP active site. We show that the α-helical conformation of the substrate is important not only during its initial interaction with MPP (i.e. substrate recognition), but also later, at...
3

Molecular Study of Interactions between Hematopoietic Stem Cells and Stromal Cells

Luo, Biao, Meng-Ling, Choong, Heard, Amanda, Li, Zhe, Moore, Kateri, Kaiser, Chris, Lemischka, Ihor R., Yap, Miranda G.S., Lodish, Harvey F. 01 1900 (has links)
Multipotent hematopoietic stem cells (HSCs) are progenitors of all types of hematopoietic cells, and the efficient isolation and propagation of HSCs will significantly enhance our ability to manage many human disorders with bone marrow transplantation, stem cell transplantation and gene therapy. We employed "Signal Sequence Trap (SST)" method with yeast invertase to clone proteins on the surface of or secreted by stromal cells that enhance or inhibit the propagation of HSC’s in culture. AFT024, a mouse fetal liver stromal cell line that maintains stem cell activity in long-term culture, was subjected to SST analysis. We identified more than 60 signal sequences or transmembrane domain containing genes expressed by AFT024 cells. We compared their expression levels between AFT024 cells and BFC012 cells, a mouse fetal liver stromal cell line that was developed in the same way as for AFT024 cells but could not support HSC in long-term culture. Pleiotrophin, T16, Sca-1, deltalike and cytokine receptor like-1(CLF-1) are expressed significantly higher in AFT024 cells than in BFC012 cells. We recently employed Affymatrix genechip technology to study the interaction of HSCs and their microenvironment. In genechip experiments, Sca-1, deltalike, pleiotrophin and CLF-1 are among the most differentially expressed genes between AFT024 and BFC012 cells, while T16 was not represented on the chip. In addition, osteopontin, pigment epithelium-derived factor, proliferins, activin subunit, CXC chemokines GRO1 and LIX are more abundant in AFT024 cells than in BFC012 cells. Genechip technology was also applied to bone marrow stromal cell lines, including MS5, S17 and OP9 cells. Two murine multipotent hematopoietic cell lines, FDCP.mix and EML cells, were also analyzed. Data from these experiments are presented. / Singapore-MIT Alliance (SMA)
4

Odorant binding protein and olfactory receptors: plausible role as detectors in an odorant biosensor / Ett luktbindande proteins och luktreceptorers möjliga roll som detektorer i en biosensor

Bengtsson, Linda January 2011 (has links)
The development of an inexpensive, portable, stable, sensitive and selective biosensor for detection of odorants is a daunting task. Here, we hypothesized the development of a detector layer composed of the protein groups; the olfactory receptors (ORs) and the odorant binding proteins (OBPs), known to bind odorants in animal sensing. We report the design of 13 OR gene-vector constructs, and their subsequent transformation into Escherichia (E.) coli (BL21 (DE3)-STAR-pLysS) strain. Moreover, we report the expression of several ORs into an in vitro wheat germ extract using three separate detergent mixes for protein solubilization.   In addition, we describe the design of an odorant binding protein from the Aenopheles gambiae mosquito PEST strain (OBP-PEST) gene-vector construct under an IPTG (Isopropyl β-D-1-thiogalactopyranoside) inducible promoter. OBP-PEST was heterologously expressed in E.coli with an 8 amino acid long sequence (WSPQFEK) attached C-terminally, via a thrombin cleavage site and a flexible linker (GSSG). The WSPQFEK sequence, commonly referred to as a Strep-tag, enabled subsequent affinity chromatography purification of the protein, via binding to an engineered Streptavidin equivalent. Surprisingly, the OBP-PEST was found to contain a signal sequence leading to its truncation and secretion when expressed in E.coli.   Biophysical analyses were established using Circular Dichroism (CD) for the analysis of two lipocalins: Beta-lactoglobulin (BLG) and OBP-PEST. We studied the solubility, refoldability and the conformational transitions of BLG, as a result of change in solvent, pH and temperature. The secondary structure of OBP-PEST and its thermal stability was investigated.   In conclusion, this thesis work has enabled biophysical analyses of OBP-PEST and future analogs of interest to the development of a stable protein detector layer. Although further experiments are needed to fully characterize the biophysical properties, and to find odorant substrates of OBP-PEST, it was found to be a suitable alternative to ORs in a biosensor detector layer application. More importantly, an inherent OBP-PEST signal sequence was found to mediate protein secretion when expressed heterologously in E.coli. To the best of our knowledge this is the first lipocalin discovered to be secreted upon heterologous expression in E.coli.   We hypothesize that this signal peptide could be used as a means for targeted secretion and, hence, efficient protein purification.
5

Structural characterization of the MATα prepro-peptide secretion leader in Pichia pastoris

Chahal, Sabreen 01 January 2016 (has links)
The methylotrophic yeast, Pichia pastoris, is the most successful and favored microbial eukaryotic expression system for the production of recombinant proteins for biopharmaceutical or industrial purposes. P. pastoris has the ability to produce foreign proteins at high levels extracellularly, and since it secretes few endogenous proteins, this ability eliminates the need for expensive purification costs. It also combines the ease of genetic manipulation with rapid growth to high cell densities and provides complex posttranslational modifications. The most commonly utilized secretion signal leader in P. pastoris is the MATα prepro signal leader, originally found in S. cerevisiae. However, because some proteins cannot be secreted efficiently by P. pastoris, strategies to enhance secretion efficiency have involved the modification of the MATα prepro secretion signal leader. The study focuses on using site-directed mutagenesis of specific sets of amino acids of MATα prepro secretion leader to evaluate the correlation between secondary structure and secretion level. MATα pro-HRP mutants were created, in order to analyze the export of heterologous proteins in P. pastoris. In addition, structural analysis through circular dichroism was performed on mutant MATα pro-peptides to evaluate differences in secondary structure as a result of the mutagenesis. Mutants, pSC6 (Δ57-65) and pSC7 (Δ66-70) did not generate the same HRP secretion level as Δ57-70. In addition, a new proposed model of MATα pro-peptide signal leader was created. This new model suggests that the N and C terminus of MATα pro-peptide need to be presented correctly for proper interaction with secretion machinery and for efficient protein secretion. With these analyses, optimization of secretion systems can be achieved to impact the fields of science, industry, healthcare, and economics worldwide.
6

Caractérisation d'une nouvelle voie d'adressage des protéines à la membrane externe des bactéries à Gram négatif / Characterization of a novel outer membrane protein targeting pathway in Gram negative bacteria

Rondelet, Arnaud 07 December 2012 (has links)
Le système Tat (pour Twin Arginine Translocation) exporte des protéines repliées depuis le cytoplasme vers le périplasme des bactéries. L’adressage des protéines à exporter au système Tat repose sur une séquence signal spécifique amino terminale clivée après exportation. Chez le phytopathogène Dickeya dadantii, l’homologue de pectine lyase PnlH possède une séquence signal Tat qui assure son adressage au système Tat mais qui n’est pas clivée après exportation et ancre la protéine dans la membrane externe. Chez les protéobactéries, la majorité des protéines de membrane externe sont soit des lipoprotéines soit des protéines intégrales de membrane en tonneau β. L’adressage de ces protéines à la membrane externe repose sur des voies spécifiques du type de protéine : la voie Lol pour les lipoprotéines et la combinaison des chaperons périplasmiques SurA, Skp et DegP et du complexe de membrane externe Bam (β barrel assembly machinery) pour les protéines en tonneau β. Au cours de ce travail, l’étude de l’adressage de PnlH à la membrane externe a montré que SurA se liait à la séquence signal hydrophobe de PnlH pour la protéger de l’environnement hydrophile au cours de son transit dans le périplasme. La séquence signal de PnlH (41 acides aminés) porte l’intégralité de l’information nécessaire à son adressage à la membrane externe. La nature de l’information adressant les protéines au système Tat est bien connue et dans ce travail nous nous sommes efforcés d’identifier les informations requises pour les deux dernières étapes de l’adressage de PnlH à la membrane externe : la traversée du périplasme et l’insertion dans la membrane externe. La délétion d’une région conservée comprise entre les résidus 28 et 41 de la séquence signal de PnlH affecte l’adressage de cette dernière à la membrane externe. Des substitutions des acides aminés conservés de cette région ne semblent pas affecter l’adressage de PnlH, indiquant que l’information nécessaire à l’adressage de PnlH à la membrane externe après exportation ne réside pas dans la séquence en acides aminés de la séquence signal de PnlH. En revanche, nos données suggèrent que la présence d’une hélice α hydrophobe dans la séquence signal de PnlH est importante pour son adressage à la membrane externe. Cette observation est particulièrement intéressante puisqu’une telle structure est généralement considérée comme une caractéristique des protéines de membrane interne. / The Twin Arginine Translocation (Tat) pathway exports folded proteins from the cytoplasm to the periplasm of bacteria. The targeting of the exported proteins to the Tat pathway relies on a specific amino-terminal signal sequence, which is cleaved after exportation. In the phytopathogen Dickeya dadantii the pectin lyase homologue PnlH is exported by the Tat pathway without cleavage of its signal sequence, which anchors PnlH into the outer membrane. In proteobacteria, the vast majority of outer membrane proteins consists of β-barrel proteins and lipoproteins. Targeting of these proteins to the outer membrane relies on two pathways: the periplasmic chaperones SurA, Skp and DegP work together with the β-Barrel-Assembly Machinery (Bam) to target and insert β-barrel proteins into the outer membrane while the Lol pathway targets and insert lipoproteins. In this work, we showed that SurA binds to the hydrophobic PnlH signal sequence during the course of its periplasmic transit. The PnlH signal sequence (41 residues) carries all the information necessary to the targeting of PnlH to the outer membrane. The nature of the information that targets proteins to the Tat system is well charcterized. Thus, we focused on the nature of the information carried by the PnlH signal sequence and that allows its crossing of the periplasm and its insertion in the outer membrane. The deletion of a conserved region of the PnlH signal sequence between residues 28 and 41 strongly affects the targeting of PnlH to the outer membrane. None of the single amino acid substitutions constructed in this region obviously affected the targeting of PnlH, indicating that the information may not reside in the amino acid sequence of the PnlH signal sequence. Consistently, our data suggest that the presence in the PnlH signal sequence of an α helix with a hydrophobic cluster is important for the targeting of PnlH to the outer membrane. This observation is striking since such a structure is considered as an inner membrane protein property.
7

Structures of protein targeting complexes

Halic, Mario 27 April 2006 (has links)
Sowohl die kotranslationale Translokation von sekretorischen Proteinen durch die Membran als auch die Insertion von Membranproteinen sind essentielle Prozesse in allen lebenden Zellen. Sie erfordern die Sortierung des translatierenden Ribosoms zur Membran mittels des Signalerkenungspartikels (SRP), eines im Verlauf der Evolution konservierten Ribonukleoprotein-Partikels. SRP erkennt die Signalsequenz einer wachsenden Proteinkette, sobald diese aus dem Ribosom hervortritt. Die Bindung von SRP führt zum Anhalten der Peptidelongation (Elongationsarrest) und zum Andocken an den membrangebundenen SRP-Rezeptor (SR). In dieser Arbeit wird die 12 Å Kryo-Elektronenmikroskopie-Struktur eines Sortierungs-Komplexes dargestellt, der aus dem Säugetier-SRP gebunden an ein aktives Ribosom mit Signalsequenz besteht. Ein erstes molekulares Modell von SRP in dieser Konformation wurde erzeugt. Es zeigt wie die S-Domäne von SRP die große ribosomale Untereinheit nahe dem Peptidtunnel-Ausgang kontaktiert, um dort die Signalsequenz zu binden. Außerdem wird deutlich wie die Alu-Domäne von SRP in die Bindungsstelle für Elongationsfaktoren hineinreicht, wodurch die Elongationsarrest-Aktivität der Alu-Domäne erklärt wird. Auf dieser Basis konnte ein erstes Struktur-basiertes Modell der ersten Schritte der kotranslationalen Proteinsortierung entworfen werden. Darüberhinaus wurde auch der Schritt des Andockens an die Membran visualisiert, indem die Struktur des Ribosom-SRP-SR-Komplexes durch Kryo-EM gelöst wurde. Erste Schlüsse hinsichtlich des Mechanismus, der das Ribosom vom SRP zum Translokon transferiert, können hier gezogen werden. Als Nebenergebnis konnte durch die erreichte hohe Auflösung die Position des wichtigen ribosomalen Proteins L30e in der Kryo-EM-Struktur des Weizenkeim-Ribosoms idenifiziert werden. / Cotranslational translocation of proteins across or into membranes is a vital process in all kingdoms of life. It requires targeting of the translating ribosome to the membrane by the signal recognition particle (SRP), an evolutionary conserved ribonucleoprotein particle. SRP recognizes signal sequences of nascent protein chains emerging from the ribosome. Subsequent binding of SRP leads to pausing of peptide elongation and docking to the membrane-bound SRP receptor. Here, the 12 Å cryo-electron microscopy structure of a targeting complex is presented consisting of mammalian SRP bound to an active 80S ribosome carrying a signal sequence. A molecular model of SRP in this functional conformation was generated. The model reveals how the S-domain of SRP contacts the large ribosomal subunit at the nascent chain exit site to bind the signal sequence, and that the Alu-domain reaches into the elongation factor binding site of the ribosome explaining its elongation arrest activity. A molecular model of the first steps of protein targeting is presented. Moreover, also the docking step has been visualized by solving a cryo-EM structure of the ribosome-SRP complex bound to the SRP receptor. This structure provides first hints regarding the mechanism of ribosome transfer to the translocon. As a side result the position of the functionally significant ribosomal protein L30e has been identified in the high resolution maps of the wheat germ ribosome.

Page generated in 0.0449 seconds