Revealing Secrets of Synaptic Protein Interactions : A Biosensor based Strategy

Seeger, Christian

January 2014

Protein interactions are the basis of synaptic function, and studying these interactions on a molecular level is crucial for understanding basic brain function, as well as mechanisms underlying neurological disorders. In this thesis, kinetic and mechanistic characterization of synaptic protein interactions was performed by using surface plasmon resonance biosensor technology. Fragment library screening against the reverse transcriptase of HIV was included, as it served as an outlook for future drug discovery against ligand-gated ion channels. The protein-protein interaction studies of postsynaptic Ca2+ -binding proteins revealed caldendrin as a novel binding partner of AKAP79. Caldendrin and calmodulin bind and compete at similar binding sites but their interactions display different mechanisms and kinetics. In contrast to calmodulin, caldendrin binds to AKAP79 both in the presence and absence of Ca2+ suggesting distinct in vivo functional properties of caldendrin and calmodulin. Homo-oligomeric β3 GABAA receptors, although not yet identified in vivo, are candidates for a histamine-gated ion channel in the brain. To aid the identification of the receptor, 51 histaminergic ligands were screened and a unique pharmacology was determined. A further requirement for identifying β3 receptors in the brain, is the availability of specific high-affinity ligands. The developed biosensor assay displayed sufficient sensitivity and throughput for screening for such ligands, as well as for being employed for fragment-based drug discovery. AMPA receptors are excitatory ligand-gated ion channels, involved in synaptic plasticity, and modulated by auxiliary proteins. Previous results have indicated that Noelin1, a secreted glycoprotein, interacts with the AMPA receptor. By using biochemical methods, it was shown that Noelin1 interacts directly with the receptor. The kinetics of the interaction were estimated by biosensor analysis, thereby confirming the interaction and suggesting low nanomolar affinity. The results provide a basis for functional characterization of a novel AMPA receptor protein interaction. The results demonstrate how secrets of synaptic protein interactions and function were revealed by using a molecular based approach. Improving the understanding of such interactions is valuable for basic neuroscience. At the same time, the technical advancements that were achieved to study interactions of ligand-gated ion channels by surface plasmon resonance technology, provide an important tool for discovery of novel therapeutics against these important drug targets.

Surface plasmon resonance

biosensor

AMPA receptor

GABAA receptor

ligand-gated ion channel

A-kinase anchoring protein

caldendrin

calmodulin

HIV

fragment based drug discovery

Dynamic Systems: Evaluation, Screening and Synthetic Application

Sakulsombat, Morakot

January 2011

The research work reported in the thesis deals with the development of dynamic covalent systems and their applications in evaluation and screening of protein-ligands and enzyme inhibitors, as well as in synthetic methodologies. The thesis is divided into four parts as described below. In part one, synthetic methodologies to access 3-functionalized phthalides and 3-thioisoindolinones using the concept of cascade reactions are demonstrated. Efficient syntheses of the target products are designed and performed in one-pot process under mild reaction conditions.  In part two, phosphine-catalyzed disulfide metathesis for the generation of dynamic carbohydrate system in aqueous solution is demonstrated. In the presence of biological target (Concanavalin A), the optimal dynamic ligand is successfully identified in situ by the 1H STD-NMR spectroscopy. In part three, lipase-catalyzed resolutions of dynamic reversible systems using reversible cyanohydrin and hemithioacetal reactions in one-pot processes are demonstrated. The dynamic systems are generated under thermodynamic control in organic solution and subsequently resolved by lipase-mediated resolution under kinetic control. The resolution processes resulted in the lipase-selected substrates with high structural and stereochemical specificities. In the last part, dynamic fragment-based strategy is presented using β-galactosidase as a model target enzyme. Based on our previous study, the best dynamic inhibitor of β-galactosidase was identified using 1H STD-NMR technique from dynamic hemithioacetal systems. The structure of the dynamic inhibitor is tailored by fragment linking and optimization processes. The designed inhibitor structures are then synthesized and tested for inhibition activities against β-galactosidase. / QC 20110526

Organic chemistry

Organisk kemi

Discovery and evaluation of direct acting antivirals against hepatitis C virus

Abdurakhmanov, Eldar

January 2015

Until recently, the standard therapy for hepatitis C treatment has been interferon and ribavirin. Such treatment has only 50% efficacy and is not well tolerated. The emergence of new drugs has increased the treatment efficacy to 90%. Despite such an achievement, the success is limited since the virus mutates rapidly, causing the emergence of drug resistant forms. In addition, most new drugs were developed to treat genotype 1 infections. Thus, development of new potent antivirals is needed and drug discovery against hepatitis C is continued. In this thesis, a FRET-based protease assay was used to evaluate new pyrazinone based NS3 protease inhibitors that are structurally different to the newly approved and currently developing drugs. Several compounds in this series showed good potencies in the nanomolar range against NS3 proteases from genotype 1, 3, and the drug resistance variant R155K. We assume that these compounds can be further developed into drug candidates that possess activity against above mentioned enzyme variants. By using SPR technology, we analyzed interaction mechanisms and characteristics of allosteric inhibitors targeting NS5B polymerases from genotypes 1 and 3. The compounds exhibited different binding mechanisms and displayed a low affinity against NS5B from genotype 3. In order to evaluate the activity and inhibitors of the NS5B polymerase, we established an SPR based assay, which enables the monitoring of polymerization and its inhibition in real time. This assay can readily be implemented for the discovery of inhibitors targeting HCV. An SPR based fragment screening approach has also been established. A screen of a fragment library has been performed in order to identify novel scaffolds that can be used as a starting point for development of new allosteric inhibitors against NS5B polymerase. Selected fragments will be further elaborated to generate a new potent allosteric drug candidate. Alternative approaches have successfully been developed and implemented to the discovery of potential lead compounds targeting two important HCV drug targets.

Direct acting antivirals

Hepatitis C

NS3-4A protease

NS5B polymerase

structure-based drug discovery

fragment-based drug discovery

surface plasmon resonance

Conception, synthèse et évaluation biologique d'inhibiteurs des protéines de la famille Bcl-2 à visée anticancéreuse : applications aux cancers de l'ovaire chimiorésistants / Design, synthesis and biological evaluation of anti-cancer inhibitors targeting Bcl-2 proteins : applications to chemoresistant ovarian cancers

Denis, Camille

21 November 2018

Les interactions protéine-protéine (IPPs) contrôlent de nombreux processus physiologiques importantsdans les cellules humaines. Une caractéristique des cancers est l'échappement des cellules àl'apoptose, qui est souvent associé à la surexpression de protéines anti-apoptotiques, membres de lafamille de protéines Bcl-2. Cette famille comprend des membres anti-apoptotiques (Bcl-2, Bcl-xL,Mcl-1) et pro-apoptotiques. Dans de nombreux cancers dont les cancers de l’ovaire chimiorésistants,l'équilibre entre les membres pro- et anti-apoptotiques de la famille de protéines Bcl-2 est altéré etconduit à la survie des cellules cancéreuses. Une des stratégies envisagées pour surmonter cettechimiorésistance est rétablir l’apoptose par l’inhibition concomitante des protéines Mcl-1 et Bcl-xL.L’objectif est de concevoir des inhibiteurs à dualité d’action visant les protéines Mcl-1 et Bcl-xL.Les travaux antérieurs du laboratoire ont permis la découverte d’un inhibiteur sélectif de la protéineMcl-1, appelé Pyridoclax. Par une approche combinant les méthodes de Fragment-Based Drug Designet Structure-Based Drug Design, à partir de la structure du Pyridoclax, la conception de dual inhibiteurs,leur synthèse et leur évaluation biologique, sont rapportées dans cette thèse. L’exploration de nouveauxespaces chimiques et biologiques est ainsi rendue possible par la mise en oeuvre de cette approche ausein de laquelle le développement de nouvelles méthodologies de synthèse dans le but de concevoirdes fragments tridimensionnels originaux sera présenté.Ces travaux de thèse ont permis de concevoir, synthétiser et caractériser plus de 90 molécules.Certaines ont montré une activité pro-apoptotique intéressante en inhibant les protéines Mcl-1 et Bcl-xLnotamment. / Protein-protein interactions (PPIs) control many important physiological processes within human cells.A hallmark of cancers is the escape of cells from apoptosis, which is often associated with theoverexpression of the anti-apoptotic proteins of the Bcl-2 family. This family comprises pro-survival(Bcl-2, Bcl-xL, Mcl-1) and pro-apoptotic members. In many cancers and, in particular, chemoresistantovarian cancers, the balance between the pro- and anti-apoptotic Bcl-2 family members is alteredleading to the survival of cancerous cells. One of the strategies used to overcome chemoresistance isto re-establish apoptosis by the concomitant inhibition of Mcl-1 and Bcl-xL proteins. Therefore, theobjective is to design dual Mcl-1/Bcl-xL inhibitors.Our groups previous work allowed the discovery of a selective Mcl-1 inhibitor, named Pyridoclax. UsingFragment-Based Drug Design and Structure-Based Drug Design approaches, from the structure ofPyridoclax, the design, synthesis and biological evaluation of dual inhibitors are reported in this thesis.The exploration of novel chemical and biological space is possible by the implementation of thisapproach. The development of synthetic methodologies for the design of new 3-dimensional fragmentswill be presented.In this work, around 90 molecules were synthesized using an approach which combined Fragment-Based Drug Design and Structure-Based Drug Design methods. Some showed a pro-apoptotic activityby inhibiting Mcl-1 and Bcl-xL proteins.

Suzuki-Miyaura

Friedel-Crafts

Bcl-xL

Modélisation moléculaire

Ovary

Fragment-Based Drug Design

Structure-Based Drug Design

Molecular modeling

Cancer

Organic chemistry

Fragment-screening by X-ray crystallography of human vaccinia related kinase 1

Ali Rashid Majid, Yousif

January 2020

Fragment-screening by X-ray crystallography (XFS) is an expensive and low throughput fragment drug discovery screening method, and it requires a lot of optimization for each protein target. The advantages with this screening method are that it is very sensitive, it directly gives the three-dimensional structure of the protein-fragment complexes, and false positives are rarely obtained. The aim of this project was to help Sprint Bioscience assess if the advantages with XFS outweigh the disadvantages, and if this method should be used as a complement to their differential scanning fluorimetry (DSF) screening method. An XFS campaign was run using the oncoprotein vaccinia related kinase 1 (VRK1) as a target protein to evaluate this screening method. During the development of the XFS campaign, a diverse fragment library was created which consisted of 298 fragments that were all soluble in DMSO at 1 M concentration. The crystallization of the protein VRK1 was also optimized in this project to get a robust, high throughput crystallization set up which generated crystals that diffracted at higher resolution than 2.0 Å when they were not soaked with fragments. The soaking protocol was also optimized in order to reduce both the steps during the screening procedure and mechanical stress caused to the crystals during handling. Lastly, the created fragment library was used in screening VRK1 at 87.5 mM concentration with XFS. 23 fragment hits could be obtained from the X-ray crystallography screening campaign, and the mean resolution of the crystal structures of the protein-fragment complexes was 1.87Å. 11 of the 23 fragment hits were not identified as hits when they were screened against VRK1 using DSF. XFS was deemed as a suitable and efficient screening method to complement DSF since the hit rate was high and fragments hits could be obtained with this method that could not be obtained with DSF. However, in order to use this screening method a lot of time needs to be spent in optimizing the crystal system so it becomes suitable for fragment screening. Sprint Bioscience would therefore need to evaluate the cost/benefit ratio of using this screening method for each new project.

Fragment based drug discovery

X-ray crystallography

screening

vaccinia related kinase 1

crystal optimization

fragment library design

differential scanning fluorimetry

Sprint Bioscience

Biochemistry and Molecular Biology

Biokemi och molekylärbiologi

Multiple Ligand Simultaneous Docking (MLSD) and Its Applications to Fragment Based Drug Design and Drug Repositioning

Li, Huameng

06 January 2012

No description available.

Bioinformatics

Biomedical Research

Biophysics

Molecular Biology

Molecular Chemistry

Pharmacology

multiple ligand simultaneous docking

MLSD

fragment based drug design

STAT3

GP130

Drug Repositioning

PSO

Synthèse d'inhibiteurs de l'interaction entre la protéine à domaine PDZ, PSD-95 et le récepteur de la sérotoninte 5-HT2A pour le traitement des douleurs neuropathiques / Inhibitors synthesis of the interaction between the PDZ domain protein, PSD-95, and the serotonin receptor 5-HT2A, for the treatment of neuropathic pain

Vallon, Gary

15 January 2016

Les protéines à domaines PDZ sont impliquées dans des interactions protéine-protéine (IPP) et participent aux transports de signaux impliqués dans de nombreuses pathologies (cancer, mucoviscidose, douleur,…). L’interruption de l’interaction entre la protéine à domaine PDZ, PSD-95, et le récepteur de la sérotonine, 5-HT2A, réduit l’hyperalgie mécanique sur un modèle expérimental de douleur neuropathique chez les rats. Afin de concevoir de nouveaux inhibiteurs de cette interaction, antalgiques potentiels, trois stratégies ont été développées au cours de ces travaux. Une première stratégie a consisté à réaliser une étude de relation structure-activité à partir d’un inhibiteur connu, qui nous a permis d’identifier des groupements pharmacophores et ainsi obtenir une nouvelle molécule possédant un noyau indolique, capable d’inhiber l’interaction entre PSD-95 et 5-HT2A et possédant un effet anti-hyperalgique chez le rat neuropathique. La deuxième stratégie a consisté à valider la méthode du fragment-based drug design aux protéines à domaines PDZ en réalisant la déconstruction d’un inhibiteur connu de l’interaction en plusieurs fragments qui ont été criblés par RMN HSQC 1H-15N. Une évaluation systématique par RMN de chaque couple de fragments, suivie d’une étude de modélisation moléculaire a ensuite permis de mettre en évidence trois nouvelles molécules qui ont été synthétisées et évaluées par RMN HSQC 1H-15N. La troisième stratégie a été une approche peptidomimétique à partir de l’extrémité C-terminale de 5-HT2A, qui a conduit à la synthèse d’un peptoïde capable d’interagir avec la protéine à domaine PDZ. Ces études nous permettent d’envisager le développement de nouveaux antalgiques soit issus de la synthèse organique soit issus de mimes de peptides. / PDZ domains proteins are involved in protein-protein interaction (PPI) and participate in the transport of signals involved in numerous diseases (cancer, cystic fibrosis, pain, …). The disruption the interaction between the PDZ domains protein, PSD-95, and the serotonin receptor, 5-HT2A, reduces mechanical hyperalgesia in a rodent model of neuropathic pain in rats. To design new inhibitors as potential analgesics of this interaction, three strategies have been developed in this work. A first strategy was to conduct a study of structure-activity relationship from a known inhibitor, which allowed us to identify the pharmacophore groups and obtain a new molecule with an indole ring, capable of inhibiting the interaction between PSD-95 and 5-HT2A and possessing an anti-hyperalgesic effect on neuropathic rats. The second strategy was to validate the method of fragment-based drug design with PDZ domains proteins by deconstruction of a known inhibitor of the interaction in several fragments which were screened by NMR HSQC 1H-15N. Systematic evaluation by NMR of each pair of fragments, followed by molecular modeling study was then used to highlight three new molecules that were synthesized, and evaluated by NMR HSQC 1H-15N. The third strategy was a peptidomimetic approach from the C-terminal of 5-HT2A receptors, which led to the synthesis of a peptoid able to interact with the PDZ domain protein. These studies allow us to consider the development of new analgesics either from organic synthesis or from peptide mimetics.

Protéines à domaines PDZ

Récepteur de la sérotonine 5-HT2A

Relation Structure Activité

Fragment-based drug design

Modélisation moléculaire

Synthèse organique multi-étapes

Douleur

PDZ domains proteins

Serotonin receptor 5-HT2A

Structure Activity Relationship

Fragment-based drug design

Molecular modeling

Organic multi-step synthesis

Pain

Synthèse stéréosélective d'Hybrides de lobéline et de ligands naturels des récepteurs nicotiniques centraux à l’acétylcholine / Stereoselective synthesis of hybrids of lobeline and natural ligands of central nicotinic acetylcholine receptors

Venot, Pierre-Etienne

26 March 2015

Au cours de ce travail, nous avons développé des voies de synthèses convergentes et énantiosélectives en vue de préparer des analogues pyrrolidiniques des alcaloïdes de Lobelia comme nouveaux ligands des récepteurs nicotiniques à l’acétylcholine. Deux familles de ligands ont été réalisées par des méthodes d’élongation mono- ou bi-directionnelle basées respectivement sur des stratégies de désymétrisation précoce ou tardive au départ du succinaldéhyde.La première partie de ce manuscrit aborde la conception d’hybrides de lobéline, nicotine et d’agonistes naturels. Ces structures originales ont été obtenues diastéréosélectivement grâce à un intermédiaire commun issu d’une élongation monodirectionnelle du succinaldéhyde. Cette voie exploitera la chimie des iminiums masqués. La mise au point de cette synthèse s’est enrichie par la découverte et la valorisation d’une nouvelle famille de ligands chimériques.La seconde partie étudie la voie d’élongation bidirectionnelle basée sur des réactions de double aza-Michael suivies de la réduction désymétrisante tardive de pyrrolidines 2,5-phénacyl méso et pseudo-méso. Cette stratégie asymétrique s’inscrit dans une démarche d’économie d’atomes et d’étapes. La perspective majeure de ce travail est l’évaluation par électrophysiologie sur différents sous-types de récepteurs à l’acétylcholine d’une sélection de ligands hybrides.Les études de RSA menées sur ces familles de composés de haute homologie structurale permettront in fine d’améliorer les modèles prédictifs décrivant les transitions allostériques des récepteurs nicotiniques à l’acétylcholine / During this PhD work, convergent and diastereoselective routes for the preparation of pyrrolidine Lobelia alkaloid analogues have been developed as novel neuronal nicotinic receptor ligands. Two families of ligands have been synthesized by a strategy of mono- or bi-directional elongation of the succinaldehyde including early or late desymmetrization process respectively.The first part of this manuscript is dedicated to the preparation of hybrids of lobeline, nicotine and other natural agonists. These original structures have been diastereoselectively obtained thanks to a common intermediate resulting of the mono-elongation of succinaldehyde. This synthetic pathway uses the chemistry of masked iminium. The development of this strategy has been enriched by the discovery and the valorisation of a new chimeric ligand family.The second part studies the “bidirectional” elongation route, based on a ring-closing double aza-Michael reaction followed by the desymmetrizing reduction of meso and pseudo-meso 2,5-diphenacyl pyrrolidines. This asymmetric strategy constitutes a step- and atom-economical approach. The major perspective of this work is the biological evaluation of selected ligands by electrophysiology made on different nAChR subtypes.The SAR studies realized on these structurally homologue ligand families could allow the improvement of the predictive molecular models describing the allosteric conformations of the nAChRs.

Aza-Michael

Oxazolopyrrolidine

Iminium

Réduction désymétrisante

Alcaloïdes de Lobelia

Hybrides

Approche par fusion de fragments

Aza-Michael

Oxazolopyrrolidine

Iminium

Desymmetrizing reduction

Lobelia alkaloids

Hybrids

Merging

Fragment based drug design (FBDD)

Découverte d'inhibiteurs de la dihydrofolate réductase R67 impliquée dans la résistance au triméthoprime

Bastien, Dominic

08 1900

No description available.

Design à base de fragments

Criblage virtuel

Arrimage moléculaire

Découverte de médicaments

Dihydrofolate réductase R67

Résistance bactérienne

Triméthoprime

Inhibition enzymatique

Fragment based design

Virtual screening

Molecular docking

Drug discovery

R67 dihydrofolate reductase

Bacterial resistance

Trimethoprim

Enzymatic inhibition

Découverte d'inhibiteurs de la dihydrofolate réductase R67 impliquée dans la résistance au triméthoprime.

Bastien, Dominic

08 1900

Le triméthoprime (TMP) est un antibiotique communément utilisé depuis les années 60. Le TMP est un inhibiteur de la dihydrofolate réductase (DHFR) bactérienne chromosomale. Cette enzyme est responsable de la réduction du dihydrofolate (DHF) en tétrahydrofolate (THF) chez les bactéries, qui lui, est essentiel à la synthèse des purines et ainsi, à la prolifération cellulaire. La résistance bactérienne au TMP est documentée depuis plus de 30 ans. Une des causes de cette résistance provient du fait que certaines souches bactériennes expriment une DHFR plasmidique, la DHFR R67. La DHFR R67 n'est pas affectée par le TMP, et peut ainsi remplacer la DHFR chromosomale lorsque celle-ci est inhibée par le TMP. À ce jour, aucun inhibiteur spécifique de la DHFR R67 est connu. En découvrant des inhibiteurs contre la DHFR R67, il serait possible de lever la résistance au TMP que la DHFR R67 confère aux bactéries. Afin de découvrir des inhibiteurs de DHFR R67, les approches de design à base de fragments et de criblage virtuel ont été choisies. L'approche de design à base de fragments a permis d'identifier sept composés simples et de faible poids moléculaire (fragments) inhibant faiblement la DHFR R67. À partir de ces fragments, des composés plus complexes et symétriques, inhibant la DHFR R67 dans l'ordre du micromolaire, ont été élaborés. Des études cinétiques ont montré que ces inhibiteurs sont compétitifs et qu'au moins deux molécules se lient simultanément dans le site actif de la DHFR R67. L'étude d'analogues des inhibiteurs micromolaires de la DHFR R67 a permis de déterminer que la présence de groupements carboxylate, benzimidazole et que la longueur des molécules influencent la puissance des inhibiteurs. Une étude par arrimage moléculaire, appuyée par les résultats in vitro, a permis d'élaborer un modèle qui suggère que les résidus Lys32, Gln67 et Ile68 seraient impliqués dans la liaison avec les inhibiteurs. Le criblage virtuel de la librairie de 80 000 composés de Maybridge avec le logiciel Moldock, et les essais d'inhibition in vitro des meilleurs candidats, a permis d'identifier quatre inhibiteurs micromolaires appartenant à des familles distinctes des composés précédemment identifiés. Un second criblage virtuel, d'une banque de 6 millions de composés, a permis d'identifier trois inhibiteurs micromolaires toujours distincts. Ces résultats offrent la base à partir de laquelle il sera possible de développer iv des composés plus efficaces et possédant des propriétés phamacologiquement acceptables dans le but de développer un antibiotique pouvant lever la résistance au TMP conféré par la DHFR R67. / Trimethoprim (TMP) is a common antibiotic which is used since the 60's. TMP is an inhibitor of the bacterial chromosomal dihydrofolate reductase (DHFR). This enzyme catalyses the reduction of the dihydrofolate (DHF) to tetrahydrofolate (THF) which is essential to the biosynthesis of purines thus to cellular proliferation. Bacterial TMP resistance is documented since about 30 years. One of the cause of this resistance comes from the fact that certain bacteria express a plasmidic DHFR, the R67 DHFR, which confers TMP resistance. The R67 DHFR is not inhibited by TMP and can replace the chromosomal DHFR when the latter is inhibited by TMP. The discovery of R67 DHFR inhibitors would allow to break the trimethoprim resistance granted by R67 DHFR. In order to discover R67 DHFR inhibitors, fragment based design and virtual screening approaches were selected. By fragment based design, seven simple compounds with a low molecular mass which inhibited weakly R67 DHFR (fragments) were identified. From these fragments, more complex and symmetrical compounds inhibiting R67 DHFR in the micromolar range were identified. Kinetic studies showed these inhibitors were competitive and at least two molecules bind simultaneously to the active site of the R67 DHFR. Test of the micromolar inhibitors analog showed that the presence of carboxylate, benzimidazole and the length of the molecule all have an effect on the potency of the inhibitors. Molecular docking of the inhibitors, supported by in vitro data, were used to develop a model which suggest that residue like Lys32, Gln67 and Ile68 would be involved in the binding of the inhibitors to the R67 DHFR. Virtual screening of the 80 000 compound Maybridge library with Moldock software, followed by in vitro test of the best candidate, identified four micromolar inhibitors which are chemically distinct from the inhibitor beforehand identified. A second virtual screening of a 6 million compounds bank identified three micromolar inhibitors which are also distinct from the inhibitor beforehand identified. vi These results offer a basis which will allow further development of more potent inhibitors with more acceptable pharmacologic properties in order to develop an antibiotic which would break the TMP resistance granted by the R67 DHFR.

Design à base de fragments

Criblage virtuel

Arrimage moléculaire

Découverte de médicaments

Dihydrofolate réductase R67

Résistance bactérienne

Triméthoprime

Inhibition enzymatique

Fragment based design

Virtual screening

Molecular docking

Drug discovery

R67 dihydrofolate reductase

Bacterial resistance

Trimethoprim

Enzymatic inhibition