Drug Partitioning into Natural and Artificial Membranes : Data Applicable in Predictions of Drug Absorption

Engvall, Caroline

January 2005

When drug molecules are passively absorbed through the cell membrane in the small intestine, the first key step is partitioning of the drug into the membrane. Partition data can therefore be used to predict drug absorption. The partitioning of a solute can be analyzed by drug partition chromatography on immobilized model membranes, where the chromatographic retention of the solute reflects the partitioning. The aims of this thesis were to develop the model membranes used in drug partition chromatography and to study the effects of different membrane components and membrane structures on drug partitioning, in order to characterize drug–membrane interactions. Electrostatic effects were observed on the partitioning of charged drugs into liposomes containing charged detergent, lipid or phospholipid; bilayer disks; proteoliposomes and porcine intestinal brush border membrane vesicles (BBMVs), and on the retention of an oligonucleotide on positive liposomes. Biological membranes are naturally charged, which will affect drug partitioning in the human body. Proteoliposomes containing transmembrane proteins and cholesterol, BBMVs and bilayer disks were used as novel model membranes in drug partition chromatography. Partition data obtained on proteoliposomes and BBMVs demonstrated how cholesterol and transmembrane proteins interact with drug molecules. Such interactions will occur between drugs and natural cell membranes. In the use of immobilized BBMVs for drug partition chromatography, yet unsolved problems with the stability of the membrane were encountered. A comparison of partition data obtained on bilayer disks with data on multi- and unilamellar liposomes indicated that the structure of the membrane affect the partitioning. The most accurate partition values might be obtained on bilayer disks. Drug partition data obtained on immobilized model membranes include both hydrophobic and electrostatic interactions. Such partition data should preferably be used when deriving algorithms or computer programs for prediction of drug absorption.

Biochemistry

Bilayer disk

Cholesterol

Drug partitioning

Drugs

Electrostatic effects

Immobilized liposome chromatography

Liposome

Membrane protein

Model membrane

Oligonucleotide-liposome complex

Phospholipid

Phospholipid bilayer

Proteoliposome

Surfactant

Biokemi

Biochemistry

Biokemi

Strukturelle und funktionelle Charakterisierung von dem mitochondrialen Membranprotein Menschlicher Spannungsabhängiger Anionen Kanal (HVDAC) und dem Membranprotein bindenden Conotoxin Conkunitzin-S1 mit Flüssigphasen NMR / Structural and functional characterisation of the mitochondrial membrane protein human voltage-dependent anion channel (HVDAC) and the membrane protein-targeting Conotoxin Conkunitzin-S1 by solution NMR

Bayrhuber, Monika

26 June 2007

No description available.

540 Chemie

Mathematics and Computer Science

Membranprotein

Apoptose

VDAC

Conotoxin

Conk-S1

NMR

Protein Strukturaufklärung

membrane protein

apoptosis

VDAC

conotoxin

Conk-S1

NMR

protein structure determination

35.25

S

Structure, Function and Dynamics of G-Protein coupled Receptors

Eichler, Stefanie

09 February 2012

Understanding the function of membrane proteins is crucial to elucidate the molecular mechanisms by which transmembrane signaling based physiological processes,i. e., the interactions of extracellular ligands with membrane-bound receptors, are regulated. In this work, synthetic transmembrane segments derived from the visual photoreceptor rhodopsin, the full length system rhodopsin and mutants of opsin are used to study physical processes that underlie the function of this prototypical class-A G-protein coupled Receptor. The dependency of membrane protein hydration and protein-lipid interactions on side chain charge neutralization is addressed by fluorescence spectroscopy on synthetic transmembrane segments in detergent and lipidic environment constituting transmembrane segments of rhodopsin in the membrane. Results from spectroscopic studies allow us to construct a structural and thermodynamical model of coupled protonation of the conserved ERY motif in transmembrane helix 3 of rhodopsin and of helix restructuring in the micro-domain formed at the protein/lipid water phase boundary. Furthermore, synthesized peptides and full length systems were studied by time resolved FTIR-Fluorescence Cross Correlation Hydration Modulation, a technique specifically developed for the purpose of this study, to achieve a full prospect of time-resolved hydration effects on lipidic and proteinogenic groups, as well as their interactions. Multi-spectral experiments and time-dependent analyses based on 2D correlation where established to analyze large data sets obtained from time-resolved FTIR difference spectra and simultaneous static fluorescence recordings. The data reveal that lipids play a mediating role in transmitting hydration to the subsequent membrane protein response followed by water penetration into the receptor structure or into the sub-headgroup region in single membrane-spanning peptides carrying the conserved proton uptake site (monitored by the fluorescence emission of hydrophobic buried tryptophan). Our results support the assumption of the critical role of the lipid/water interface in membrane protein function and they prove in particular the important influence of electrostatics, i. e., side chain charges at the phase boundary, and hydration on that function. / Für die Aufklärung der molekularen Wirkungsweise von physiologischen, auf Signaltransduktion, d. h. dem Zusammenspiel von extrazellulären Reizen und membrangebundenen Rezeptoren, beruhenden Prozessen ist das Verständnis der Funktion von Membranproteinen unerlässlich. In dieser Arbeit werden von Rhodopsin abgleitete, synthetische transmembrane Segmentpeptide, Opsin-Mutanten und der vollständige Photorezeptor Rhodopsin untersucht, um die physikalischen Prozesse zu beleuchten, die der Funktionen dieses prototypischen Klasse-A G-Protein gekoppelten Rezeptors zugrunde liegen. Die Abhängigkeit der Membranprotein-Hydratation und der Lipid-Protein-Wechselwirkung von der Ladung einer Aminosäuren-Seitenkette wird erforscht. Hierzu werden synthetische, transmembrane Segmentpeptide in Lipid und Detergenz, als Modell transmembraner Segmente von Rhodopsin in der Membran mittels Fluoreszenzspektroskopie untersucht. Aus den erhaltenen Ergebnissen wird ein thermodynamisches und strukturelles Modell hergeleitet, welches die Kopplung der Protonierung des hochkonservierten ERY-Motivs in Transmembranhelix 3 von Rhodopsin an die Restrukturierung der Helix in der Mikroumgebung der Lipid-Wasser-Phasengrenze erklärt. Des Weiteren werden sowohl die Segementpeptide als auch die vollständigen Systeme Opsin und Rhodopsin mittels zeitaufgelöster FTIR-Fluoreszenz-Kreuzkorrelations-Hydratations-Modulation untersucht. Diese Technik wurde eigens zur Aufklärung von zeitabhängigen Hydratationseffekten auf Lipide und Proteine oder Peptide entwickelt. Dabei werden zeitaufgelöste FTIR Differenz-Spektren und gleichzeitig statische Fluoreszenzsignale aufgenommen und diese zeitabhängigen multispektralen Datensätze mittels 2D Korrelation analysiert. Die Auswertung der Experimente enthüllt einen sequentiellen Hydratationsprozess. Dieser beginnt mit der Bildung von Wasserstoffbrückenbindungen an der Carbonylgruppe des Lipids, gefolgt von Strukturänderungen der Transmembranproteine und abgeschlossen durch das Eindringen von Wasser in das Proteininnere. Letzteres wird nachgewiesen durch die Fluoreszenz von Tryptophan im hydrophoben Peptid- oder Proteininneren. Die Ergebnisse dieser Arbeit unterstreichen die Annahme, dass Lipid-Protein-Wechselwirkungen eine entscheidende Rolle in der Funktion von Membranproteinen spielen und das insbesondere Elektrostatik, in Form von Ladungen an der Phasengrenze, und die Hydratisierung einen kritischen Einfluss auf diese Funktion haben.

Membranprotein

G-Protein gekoppelter Rezeptor

Lipid

Protonen

Proteinstruktur

FTIR

Fluoreszenz

membrane protein

G-protein coupled receptor

lipid

proton

protein structure

FTIR

fluorescence

ddc:570

rvk:WE 5160

Transcriptional Analysis of Chlamydial Persistence

Hogan, Richard

January 2004

Chlamydial infections have been associated with several chronic human diseases, including trachoma, pelvic inflammatory disease, chronic obstructive pulmonary disease and atherosclerotic cardiovascular disease. In Chlamydia-associated disease, the organisms are believed to exist in an atypical, persistent phase that is not well understood at the genetic level. The research presented in this thesis investigated chlamydial gene expression in in vitro cell culture models of persistence. The first set of studies analysed a continuous-infection model of persistence that has been recently developed for two C. pneumoniae isolates (TW-183 and CM-1). The spontaneous establishment and unique cyclical nature of continuous infections could be particularly relevant to in vivo events. An initial analysis using a semi-quantitative reverse transcriptase PCR (sqRT-PCR) approach provided evidence of differential gene expression in C. pneumoniae TW-183 continuous infections relative to acute control infections. Using a subsequently established fully quantitative real-time reverse transcriptase PCR (rtRT-PCR) assay, up-regulated expression profiles were confirmed for five genes (CPn0483, nlpD, ompA, pmp1 and porB) in the continuous C. pneumoniae TW-183 infections. The omcB, pmp1 and porB genes, all of which encode membrane proteins, showed similar patterns of expression over both the acute and continuous time courses tested. Gene expression data for a second C. pneumoniae isolate, CM-1, revealed similar overall expression trends to those seen for C. pneumoniae TW-183 but also supported previous observations of different growth characteristics between the two isolates in the continuous-infection model. The rtRT-PCR assay was further optimised for use in gene expression studies of the gamma interferon (IFN-γ)-mediated model of C. pneumoniae A-03 persistence, in which altered growth and morphological traits typical of chlamydial persistence have been well characterised. Meanwhile, chlamydial genes such as euo, ftsK and hctB were emerging from the literature as reliable genetic markers of persistence. Therefore, a preliminary rtRT-PCR analysis of marker gene expression was used to assess the likely extent of persistence in individual IFN-γ-treated C. pneumoniae A-03 infections from a series of experiments that had been prepared for this persistence model. In this way, an appropriate pair of duplicate experiments was selected for further studies based on strong genetic evidence of persistence in IFN-γ-treated samples at 48 h post-infection (PI) in those experiments. Using rtRT-PCR, 14 genes of interest from the related peptidoglycan, aminosugars and lipopolysaccharide (LPS) biosynthetic pathways were analysed in the validated experiments of the IFN-γ-mediated C. pneumoniae A-03 persistence model. Selective up- and down-regulated expression trends were associated with IFN-γ-treatment at 48 h PI for genes encoding products that are located at specific enzymatic points in these pathways. Most strikingly, the expression of glmU, the product of which controls the amount of an essential precursor metabolite that enters both peptidoglycan and LPS biosynthesis, was strongly and reproducibly down-regulated in the 48-h PI IFN-γ-treated samples. This expression profile may contribute to a reduced rate of peptidoglycan biosynthesis in this persistence model and may therefore be related to the inhibited cell division and RB-to-EB differentiation that characterise chlamydial persistence. While most other genes in these pathways showed unchanged expression associated with IFN-γ treatment, murA and kdsB (from peptidoglycan and LPS biosynthesis, respectively) were selectively up-regulated in the 48-h PI IFN-γ-treated samples. Taken together, these data supported the concept of a persistence stimulon in C. pneumoniae that is regulated at key points in various metabolic pathways. In addition to the analysis of biosynthetic genes, the up-regulated gene set from continuous C. pneumoniae TW-183 infections was also analysed in the validated IFN-γ-mediated C. pneumoniae A-03 persistence experiments. The data revealed similarities and differences in gene expression patterns between these two in vitro persistence models. Furthermore, the profiles obtained for genes such as pmp1 and porB provided insights into the widely predicted phenomenon of late developmental gene shut-down during chlamydial persistence. A final investigation into an analogous IFN-γ-mediated persistence system for C. trachomatis serovar L2 focussed on one up-regulated (murA) and one down-regulated (glmU) gene from the validated IFN-γ-mediated persistent C. pneumoniae A-03 data set. Both genes were significantly down-regulated in persistent C. trachomatis, adding to a growing body of evidence for key differences among chlamydial species in their persistent gene expression patterns. This project has contributed significantly to our understanding of the molecular basis of the important persistent phase of chlamydial development.

Chlamydia pneumoniae

Chlamydia trachomatis

persistence

continuous-infection model

gamma interferon

real-time PCR

RT-PCR

differential gene expression

membrane protein

peptidoglycan

Cryo-microscopie électronique des complexes de l'adressage et de la translocation co-traductionnelle chez E. coli / Electron cryo-microscopy of complexes in E. coli co-translational targeting and translocation

Jiang, Qiyang

18 June 2015

La membrane cellulaire est la barrière qui sépare l'intérieur des cellules de l'environnement extérieur. Elle se compose de lipides et de protéines. Les gènes codant pour les protéines membranaires représentent environ 30% des génomes. Les protéines membranaires sont synthétisées dans le cytosol par les ribosomes, mais suivent des voies spécifiques pour s'intégrer dans la membrane cellulaire. Les ribosomes en cours de traduction de protéines membranaires sont reconnus dans le cytosol et adressés à la membrane. Par la suite, les chaînes naissantes de protéines membranaires sont insérées dans la bicouche lipidique puis repliées de façons appropriées, ce mécanisme s'appelle la translocation. Le processus d'adressage est médiée par la particule de reconnaissance du signal (SRP) et son récepteur, tandis que la translocation est effectuée par un certain nombre de complexes de protéines membranaires.Cette thèse décrit deux des complexes impliqués dans cet adressage et translocation co-traductionnelle chez Escherichia coli : Le complexe ribosome-SRP-FtsY pour l'adressage en conformation «fermé» et le complexe dans lequel le ribosome est lié à l'holo-translocon (HTL) qui se compose de sept protéines membranaires. J'ai utilisé principalement la cryo-microscopie électronique pour caractériser ces complexes. La cryo-EM permet de déterminer la structure des échantillons biologiques à une résolution supérieure au nanomètre dans leur environnement natif, sans avoir à le cristalliser. Dans ce travail, j'ai bénéficié des améliorations récentes dans l'équipementet le traitement d'image.A partir d'un ensemble de données de cryo-EM obtenu par les membres du groupe, j‘ai déterminé la structure du complexe ribosome-SRP-FtsY en conformation «fermé» avec une résolution de 5.7 Å. Différentes stratégies de tri des calculsont été appliquées pour identifier la partie la plus homogène de l'ensemble des données. La structure montre un domaine bien résolu SRP ARN et SRP M avec une séquence signal liée. L'interaction entre les SRP et le ribosome pourrait être modélisée avec une grande fidélité. Cette structure révèle également que les GTPases SRP-ftsY sont détachées de la tétra-boucle de l'ARN et sont flexibles, libérant alors le site de sortie du ribosomepermettant la liaison du translocons.Dans le second projet, différentes approches ont été poursuivis pour résoudre la structure du complexe ribosome-HTL à haute résolution. Une structure initiale à 22 Å a été obtenue en mélangeant HTL solubilisés en détergent avec des ribosomes, démontrantla possibilité de préserver le complexe dans les conditions utilisées pour la préparation des grilles. J'ai ensuite exploré l'utilisation de nanodiscs et un nouveau détergent appelé LMNG pour stabiliser HTL dans des tampons sans détergent. Un deuxième ensemble de données a ensuite été recueilli à partir d'échantillon obtenu par gradient de fixation, la structure a été résolue à 17 Å. La préparation des échantillons a été optimisée utilisant entre autre les amphipoles. On a montré que deux types d'amphipole-HTL peuvent se lier au ribosome, et des structures de plus grande résolution devrait être obtenu à partir de ces échantillons. / The cell membrane is the barrier that separates the interior of cells from the outside environment. It consists of lipids and proteins. Genes encoding membrane proteins make up about 30% of the genome. Membrane proteins are synthesized in the cytosol by ribosomes, but employ special pathways to integrate into the cell membrane. Ribosomes translating membrane proteins are recognized by special factors in the cytosol and targeted to the membrane. Subsequently, nascent chains of the membrane proteins are inserted into the lipid bilayer and are folded into their proper structures, a process termed translocation. The targeting process is mediated by the signal recognition particle (SRP) and its receptor, while the translocation is performed by a number of membrane protein complexes.This thesis describes two of the complexes involved in co-translational targeting and translocation in Escherichia coli: The ribosome-SRP-FtsY targeting complex in the “closed” conformation and the complex of a ribosome with the holo-translocon (HTL) consisting of seven membrane proteins. I mainly used electron cryo-microscopy to characterize these complexes. Cryo-EM allows structural determination of biological samples at sub-nanometer resolution in their native environment, without the need to crystallize the specimen. In this work, I took advantage of the recent advances in both the hardware and the image processing.Starting from a cryo-EM dataset obtained by group members, I have determined the structure of ribosome-SRP-FtsY complex in the “closed” conformation at 5.7 Å resolution. Different computational sorting strategies were applied to identify the most homogeneous sub-pool of the dataset. The structure shows a well-resolved SRP RNA and SRP M domain with a signal sequence bound. The interaction between SRP and ribosome could be modeled with high confidence. This structure also reveals that the SRP-FtsY GTPases are detached from the RNA tetraloop and are flexible, thus liberating the ribosomal exit site for binding of the translocation machinery.In the second project, different approaches were pursued to solve the structure of the ribosome-HTL complex at high resolution. An initial structure at 22 Å was obtained by mixing detergent-solubilized HTL with the ribosome, demonstrating that it is possible to preserve the complex under the conditions used for specimen preparation. I have then explored the use of nanodiscs and a new detergent called LMNG to stabilize HTL in detergent-free buffers. A second dataset was subsequently collected from a sample prepared by gradient-fixation, and the structure was solved at 17 Å. Sample preparation has been optimized further using amphipols. Two types of amphipol-HTL complexes were shown to bind to the ribosome, and higher resolution structures are expected to be obtained from these samples.

Cryo-microscopie électronique

Protéine membranaire

Ribosome

Adressage des protéines

Translocation des protéines

Electron cryo-microscopy

Membrane protein

Ribosome

Protein targeting

Protein translocation

500

570

Homéostasie du cuivre dans le chloroplaste : étude comparée de deux transporteurs de la famille des ATPases de type PIB / Copper homeostasis in chloroplasts : comparative study of two transporters belonging to the PIB- type ATPases family

Sautron, Emeline

14 October 2015

Le cuivre est un métal de transition essentiel pour le fonctionnement des organismes vivants. Chez la plante Arabidopsis thaliana, la moitié du contenu en cuivre est localisé dans le chloroplaste. Cet organite, spécifique des cellules végétales, est constitué d'une enveloppe délimitant le stroma, un compartiment aqueux au sein duquel se trouve un système membranaire complexe, les thylacoïdes. Dans les chloroplastes d'Arabidopsis, le cuivre est le cofacteur de deux protéines essentielles : la superoxyde dismutase Cu/Zn, impliquée dans la défense contre des espèces réactives de l'oxygène au niveau du stroma et la plastocyanine, une protéine du lumen des thylacoïdes, impliquée dans la chaine de transfert des électrons photosynthétiques. Des études de génétique inverse ont démontré que le transport du cuivre à la plastocyanine impliquait deux protéines membranaires appartenant à la famille des ATPases-PIB-1 : HMA6, localisée dans l'enveloppe et HMA8, localisée dans la membrane des thylacoïdes. Une étude fonctionnelle in vitro a montré que HMA6 était un transporteur de haute affinité de cuivre monovalent présentant les caractéristiques générales des ATPases-P. Afin de comparer les propriétés enzymatiques de ces deux ATPases-PIB-1 et de mieux comprendre leur rôle respectif dans l'homéostasie du cuivre au sein du chloroplaste, nous avons déterminé in vitro les propriétés enzymatiques de HMA8.La stratégie employée pour la caractérisation de HMA8 a été similaire à celle utilisée pour la caractérisation de HMA6. Dans un premier temps, la sélectivité ionique de HMA8 a été évaluée à l'aide de tests phénotypiques dans la levure Saccharomyces cerevisiae. Les propriétés enzymatiques de HMA8 ont ensuite été déterminées in vitro après expression dans la bactérie Lactoccocus lactis, par des expériences de phosphorylation par l'ATP. Cette analyse a permis de démontrer que HMA8 présentait une plus forte affinité apparente pour le cuivre mais une activité catalytique plus lente que HMA6. L'analyse de modèles tridimensionnels de HMA6 et HMA8 a montré que ces différences pourraient être expliquées par des différences de charges au niveau de la cavité où le métal est libéré et/ou par la nature des partenaires interagissant avec ces ATPases. Ces différences pourraient expliquer les fonctions distinctes de ces deux transporteurs dans le chloroplaste : HMA6 régulerait la concentration en cuivre dans le stroma en interagissant avec différentes protéines cibles (notamment des chaperonnes à cuivre), alors que HMA8 aurait un rôle plus précis pour la distribution du cuivre à la plastocyanine.Pour mieux comprendre le mécanisme de libération du cuivre par HMA6 et HMA8, nous avons effectué une étude fonctionnelle de mutants de la région reliant les deux premières hélices transmembranaires (TMA et TMB). Dans cette étude, nous avons ciblé les cystéines et histidines qui de par leurs propriétés chimiques sont les résidus les plus à même d'interagir avec le métal. Les mutants d'intérêts ont été sélectionnés par criblage phénotypique dans la levure puis exprimés dans la bactérie L. lactis. La caractérisation biochimique in vitro de leurs propriétés enzymatiques a été réalisée par des tests de phosphorylation par l'ATP et le Pi. Cette étude nous a permis d'identifier deux résidus, une cystéine et une histidine, impliqués la libération du cuivre et de proposer un modèle de cheminement du métal dans la partie extracytoplasmique du site de transport de HMA6 / Copper is an essential transition metal for living organisms. In the plant Arabidopsis thaliana, half the copper content is localized in the chloroplast. This organelle specific of plant cells, consists of an envelope delimiting the stroma, an aqueous compartment within which there is a complex membrane system, the thylakoids. In chloroplasts of Arabidopsis, copper is the cofactor of two essential proteins: the superoxide dismutase Cu / Zn, involved in defense against reactive oxygen species in the stroma and plastocyanin, a protein of the thylakoid lumen involved in the chain transfer photosynthetic electron. Reverse genetics studies have demonstrated that copper transport in plastocyanin involved two membrane proteins belonging to the family of ATPases-PIB-1: HMA6, located in the envelope and HMA8, localized in the thylakoid membranes. A functional in vitro study showed that HMA6 was a monovalent high affinity copper transporter showing the general characteristics of P-ATPases. To compare the enzymatic properties of these two ATPases and better understand their respective role in copper homeostasis in the chloroplast, we in vitro determined the enzymatic properties of HMA8.The strategy employed for the characterization of HMA8 was similar to that used for the characterization of HMA6. Initially, the ion selectivity of HMA8 was evaluated using phenotypic tests in the yeast Saccharomyces cerevisiae. The enzymatic properties of HMA8 were then determined in vitro after expression in the bacterium Lactoccocus lactis, by phosphorylation experiments by ATP. This analysis demonstrated that HMA8 had a stronger apparent affinity for copper but a slower catalytic activity than HMA6. The analysis of three-dimensional models of HMA6 and HMA8 showed that these differences could be explained by differences in the electrostatic potential at the cavity where the metal is released and/or by the nature of the partners interacting with these ATPases. These differences might explain the distinct functions of the two carriers in the chloroplast: HMA6 would regulate the copper concentration in the stroma by interacting with various target proteins (including copper chaperone), while HMA8 would have a more specific role for the distribution of copper plastocyanin.To better understand the mechanism of copper release by HMA6 and HMA8, we conducted a functional study of mutants of the region connecting the first two transmembrane helices (TMA and TMB). In this study, we specifically targeted cysteines and histidines because of their chemical properties that make them very strong metal ligands. The mutants of interest were selected by phenotypic screening in yeast and then expressed in the bacterium L. lactis. The in vitro biochemical characterization of their enzymatic properties was carried out by phosphorylation tests by ATP and Pi. This study allowed us to identify two residues, one cysteine and one histidine, involved the release of copper and to propose a metal path model in extracytoplasmic part of the transport site of HMA6

ATPase-P1B

Chloroplaste

Caractérisation biochimique

Homéostasie du cuivre

Structure

Protéine membranaire

P1B-ATPase

Chloroplast

Biochemical characterization

Copper homeostasis

Structure

Membrane protein

570

580

Methods for Detection of Small Molecule-Protein Interactions

January 2015

abstract: Detection of molecular interactions is critical for understanding many biological processes, for detecting disease biomarkers, and for screening drug candidates. Fluorescence-based approach can be problematic, especially when applied to the detection of small molecules. Various label-free techniques, such as surface plasmon resonance technique are sensitive to mass, making it extremely challenging to detect small molecules. In this thesis, novel detection methods for molecular interactions are described. First, a simple detection paradigm based on reflectance interferometry is developed. This method is simple, low cost and can be easily applied for protein array detection. Second, a label-free charge sensitive optical detection (CSOD) technique is developed for detecting of both large and small molecules. The technique is based on that most molecules relevant to biomedical research and applications are charged or partially charged. An optical fiber is dipped into the well of a microplate. It detects the surface charge of the fiber, which does not decrease with the size (mass) of the molecule, making it particularly attractive for studying small molecules. Third, a method for mechanically amplification detection of molecular interactions (MADMI) is developed. It provides quantitative analysis of small molecules interaction with membrane proteins in intact cells. The interactions are monitored by detecting a mechanical deformation in the membrane induced by the molecular interactions. With this novel method small molecules and membrane proteins interaction in the intact cells can be detected. This new paradigm provides mechanical amplification of small interaction signals, allowing us to measure the binding kinetics of both large and small molecules with membrane proteins, and to analyze heterogeneous nature of the binding kinetics between different cells, and different regions of a single cell. Last, by tracking the cell membrane edge deformation, binding caused downstream event – granule secretory has been measured. This method focuses on the plasma membrane change when granules fuse with the cell. The fusion of granules increases the plasma membrane area and thus the cell edge expands. The expansion is localized at the vesicle release location. Granule size was calculated based on measured edge expansion. The membrane deformation due to the granule release is real-time monitored by this method. / Dissertation/Thesis / Doctoral Dissertation Electrical Engineering 2015

Electrical engineering

Biomedical engineering

Chemical engineering

Binding kinetics measurement

Charge sensitive detection method

Drug screening

Label free detection methods

Vesicle release

Etude fonctionnelle du coeur catalytique membranaire d'enzymes de la famille NOX : Identification de la première NADPH oxydase procaryote / Functional studies of the membranous cataltytic core of NOX family enzymes : Identification of the first prokaryotic NADPH oxidase

Hajjar, Christine

21 November 2014

La famille des NADPH oxydases est constituée de complexes multi protéiques, dont un des composants est la sous unité catalytique NOX. Il s'agit de protéine transmembranaire qui assure le transport des électrons à travers la membrane, à partir d'un donneur d'électrons, le NADPH, à un accepteur final, l'oxygène moléculaire. Il en résulte la production de superoxydes, précurseur d'espèces réactives de l'oxygène. Les NOX sont impliquées dans divers processus physiologiques et pathologiques qui les ont placés au rang des cibles thérapeutiques à forte valeur ajoutée.Les NOX sont reportées comme des protéines membranaires propres aux eucaryotes supérieures. Ainsi toutes les données fonctionnelles disponibles pour cette famille d'enzyme, ont été le fruit des études structure-fonction et de données putatives indirectes. D'où l'idée et l'intérêt d'identifier chez les procaryotes des candidats homologues aux Nox eucaryotes et susceptibles d'être de bons modèles pour des études structurales. En se servant d'outils bio-informatiques, nous avons définis des signatures de séquences propres aux NOX et avons identifié chez les procaryotes des centaines de séquences homologues. SpNox de chez Streptococcus Pneumoniae, a été sélectionnée et surexprimée chez E. Coli. SpNox a été purifiée et a fait l'objet d'une caractérisation fonctionnelle et biochimique approfondie. Au vue des résultats obtenus, SpNox se rapproche de part ses propriétés structurales et mechanistiques des NOX eucaryotes. Ainsi elle se présente comme le premier modèle procaryote de protéine NOX. Les premiers cristaux de cette famille de protéines ont été obtenus et son rôle in vivo reste à exploiter.En parallèle à l'approche procaryote, nous avons mené une étude structure-fonction sur la protéine NOX2 des neutrophiles PLB-985. Deux arginines conservées chez toutes les NOX eucaryotes ont été sélectionnées et leur rôle a été étudié par mutagenèse dirigée. Apres évaluation des propriétés enzymatiques des mutants NOX2, nous avons pu identifier l'arginine 513 comme étant impliquée dans la spécificité de NOX2 vis a vis du NADPH. Ces résultats nous ont permis de proposer une nouvelle orientation du NADPH dans son site d'ancrage à la protéine NOX2. / The NADPH oxidase complex was the first identified example of a system that generates reactive oxygen species in a dedicated manner. NOX are proteins involved in the transmembrane transfer of electrons to the molecular oxygen, resulting in the production of superoxides. In addition to ROS related damages, deregulation of Nox-dependant ROS production induces pathological consequences. Accordingly, the Nox family became a potential drug target, making the understanding of their function at molecular basis crucial.In the literature, it has always been reported that Nox proteins exist only in eukaryotes. Since eukaryotic membrane proteins have proven to be difficult to study, all the data available on Nox enzymes are obtained from putative assignments or structure-function studies.In our project, to overcome the difficulty of working on eukaryotic membrane proteins, we used an original approach based on bioinformatics tools. Through using specific filters and a novel program, we were able to identify hundreds of prokaryotic candidates. Among them, we selected SpNox, as a prokaryotic model from Streptococcus Pneumoniae. We have developed its expression in E. Coli as well as a multistep purification scheme. We also conducted an extensive enzymatic and mechanistic characterization of the purified enzyme. Our data support a strong structural and functional homology with known NOX enzymes. Finally, crystallization trials are performed leading to first crystals ever obtained for this family of protein. The understanding of Nox's physiological function in bacteria remains to investigate.In parallel to the prokaryotic approach, a structure-function study was conducted on the human model NOX2 in the PLB-985 neutrophils. Conserved arginines among eukaryotic Nox sequences were selected. Site directed mutagenesis followed by activity tests, lead us to identify a crucial role for arginine 513. It is implicated in the specificity towards NADPH as an electron donor for NOX2. With these data, we were able to suggest a new orientation of the NADPH, notably the phosphate moiety, in the binding site.

Protéine membranaire

Flavocytochrome

Proteine recombinante

Procayote

Crystallogenese

Espèce réactive de l'oxygène

Membrane protein

Flavocytochrome

Flavocytochrome

Recombinant protein

Prokaryote

Crystallogenesis

Reactive oxygen species

540

Caractérisation de l'état oligomérique du transporteur mitochondrial ADP/ATP dans des membranes natives / Probing the oligomeric organization of the mitochondrial ATP/ADP carrier in native membranes.

Moiseeva, Vera

12 June 2012

Le passage sélectif de molécules à travers la membrane interne des mitochondries est essentiel aux processus métaboliques des cellules eucaryotes. Cette communication cellulaire est assurée par des protéines transmembranaires de la famille des transporteurs mitochondriaux (MCF). Le transporteur ADP/ATP (AAC) est le membre le plus connu et le mieux caractérisé de cette famille. Il est responsable de l'import d'ADP dans la matrice mitochondriale et de l'export d'ATP après synthèse vers le cytosol. La structure d'AAC est connue mais plusieurs questions restent ouvertes concernant le mécanisme du transport, la sélectivité et l'état oligomérique, controversé, de la protéine. Pendant plusieurs années des études biochimiques réalisées sur la protéine solubilisée en détergent étaient en faveur d'une organisation dimérique du transporteur, mais la structure d'AAC, monomérique a remis en cause ce dogme. Afin de caractériser l'organisation oligomérique d'AAC in vivo, nous avons combiné plusieurs approches. Nous avons réalisé des expériences de FRET (Fluorescence Resonance Energy Transfer) directement sur des cellules mammifères ou bactériennes (E. coli) surexprimant la protéine AAC fusionnée avec des sondes FRET. En parallèle, nous avons mis au point des tests fonctionnels afin de contrôler l'état des mitochondries et l'activité du transporteur dans ces cellules. Enfin nous avons étudié la stoechiométrie de liaison de l'inhibiteur carboxyatractyloside grâce à des mesures de respiration sur des mitochondries extraites de foie de rat et placées dans différents états métaboliques. L'ensemble des résultats présentés dans ce manuscrit ont permis de montrer que 1) l'unité fonctionnelle d'AAC est monomérique 2) l'organisation structurale d'AAC dans les membranes natives dépend de l'état métabolique des mitochondries et peut être associée à des phénomènes de régulation. / The transport of small molecules through the inner mitochondrial membrane is essential in eukaryotic metabolism and is selectively controlled by a family of integral membrane proteins, the Mitochondrial Carrier Family (MCF). The ADP/ATP carrier (AAC), which is responsible for the import of ADP to the matrix of mitochondria and the export of newly synthesized ATP toward the cytosol, is the best-known and characterized MCF member. Although its structure sheds light on several aspects of the carrier activity, additional investigations are still required to decipher the whole transport mechanism, to understand the specificity and to characterize the controversial oligomeric state of the protein. For many years, based on studies mainly carried on detergent solubilized AAC the general consensus has been in favor of a dimeric organization of the carrier. The AAC three-dimensional structure, monomeric, broke this dogma. In order to get a precise insight into the in vivo oligomeric organization of AAC we combined several approaches. Fluorescence resonance energy transfer (FRET) measurements were performed directly on mammalian and E.coli cells expressing AAC labeled with several types of FRET probes. In parallel, different functional assays were established to control the state of the mitochondria in these cells and the transport activity of these AAC fusions. Lastly, measurements of the respiration rate coupled to the titration of the inhibitory effect of carboxyatractyloside on isolated rat liver mitochondria were used to investigate the organization of AAC in native mitochondria within two regimes of oxidative phosphorylation. Taken together the results described herein revealed that 1) AAC can function mechanistically as a monomer, 2) the organization of AAC in native membranes might be related to the state of the mitochondria and be involved in regulation.

Transporteurs mitochondriaux

Transporteur ADP/ATP

FRET

Protéine membranaire

Etat oligomérique

Tests fonctionnels

Mitochondrial carrier

ADP/ATP carrier

FRET

Membrane protein

Oligomeric state

Functional assays

Estudos estruturais e funcionais de diidroorotato desidrogenases / Structural and functional studies of dihydroorotate dehydrogenase

Sheila Gonçalves do Couto Carvalho

28 March 2008

As enzimas diidroorotato desidrogenases (DHODHs) são flavo-enzimas que catalisam a oxidação do diidroorotato em orotato na quarta etapa da biossíntese de novo de nucleotídeos de pirimidina. Durante a rápida proliferação celular em mamíferos, a via de salvação de pirimidinas é insuficiente para suprir deficiências na síntese de nucleotídeos. Além disso, certos parasitas não possuem a via de salvação e contam somente com a biossíntese de novo para a produção de nucleotídeos. Por esta razão, DHODH se tornou um excelente alvo na busca por inibidores que interrompam a síntese de nucleotídeos. As enzimas DHODHs de E. coli (EcDHODH) e de X. fastidiosa (XfDHODH) são membros da classe 2 das DHODHs e encontram-se associadas à membrana citoplasmática através de uma extensão em seu N-terminal, enquanto que DHODH de T. cruzi (TcDHODH), membro da classe 1 de DHODHs, é uma proteína citosólica. Neste trabalho, usamos uma combinação de metodologias de biologia molecular e bioquímica com técnicas espectroscópicas para obter informações estruturais e funcionais acerca da enzima DHODH. Assim, Ressonância Paramagnética Eletrônica (RPE) associada à marcação de spin sítio dirigida (SDSL) e simulação espectral foram empregadas para estudar a interação da EcDHODH com modelos de membrana. Mudanças na dinâmica estrutural das vesículas induzidas pela enzima foram monitoradas via marcadores de spin localizados em diferentes posições ao longo da cadeia acil de fosfolipídios. Além disso, técnicas de DNA recombinante e mutações sítio dirigidas foram utilizadas para produzir mutantes de EcDHODH no qual um sondas paramagnéticas foram seletivamente ligadas em resíduos localizados na extensão N-terminal da proteína para experimentos subseqüentes de RPE-SDSL. Esses são os primeiros experimentos de marcação de spin sítio dirigida realizados no Brasil e com os quais monitoramos a dinâmica experimentada na região do N-terminal. Além disso, várias tentativas foram feitas para se expressar e purificar a enzima XfDHODH e a estabilidade estrutural da enzima TcDHODH na presença de um de seus inibidores naturais, o orotato, foi monitorada através de experimentos de Dicroísmo Circular (CD). / Dihydroorotate dehydrogenases (DHODHs) are flavin-containing enzymes which catalyse the conversion of (S)-dihydroorotate to orotate, in the fourth step of the de novo biosynthesis of pyrimidine nucleotides. In rapidly proliferating mammalian cells, pyrimidine salvage pathway is insufficient to overcome deficiencies for nucleotide synthesis. Moreover certain parasites lack salvage enzymes, relying solely on the de novo pathway to produce nucleotides. Thus, DHODH has turned out an excellent target to the development of inhibitors that block nucleotide biosynthesis. E. coli DHODH (EcDHODH) and X. fastidiosa DHODH (XfDHODH) are class 2 DHODHs found associated to cytosolic membranes through an N-terminal extension, whereas T. cruzi DHODH (TcDHODH) is a class 1 DHODH localizated in the cytoplasm. In the present work, we used a combination of molecular biology and biochemical methodologies with spectroscopic techniques to obtain structural and functional information on DHODH. On one hand, Electronic Paramagnetic Resonance (EPR) associated with Site-directed Spin Labeling (SDSL) and spectral simulation were employed to study the interaction of EcDHODH with vesicles. Changes in vesicle dynamic structure induced by the enzyme were monitored via spin labels located at different positions along the phospholipid acyl chain and via spin labels located at enzyme specific positions. On the other hand, DNA techniques and site-directed mutagenesis were used to produce mutants of EcDHODH where a nitroxide spin probe was selectively attached to some residues located at the protein N-terminal extension for subsequent EPR-SDSL experiments. These are the first site-directed spin labeling experiments performed in Brazil and the spectra allowed us to monitor dynamics experienced by those residues at the EcDHODH N-terminal domain. Furthermore, molecular biology and biochemical assays were employed with the objective of expressing and purifying XfDHODH and Circular Dichroism (CD) was utilized to probe the structural stability of TcDHODH in the presence of its natural inhibitor (orotate).

Diidroorotato desidrogenase

Interação proteína-membrana

Marcação de spin sítio dirigida

Relação estrutura-função

Dihydroorotate dehydrogenase

Membrane-protein inteaction

Site-directed spin labeling

Structure-function relationship