Rôle différentiel des isoformes de PML en réponse au trioxyde d’arsenic et dans la défense antivirale / Differencial role of PML isoforms in arsenic trioxyde response and in antiviral defense

El Asmi, Faten

13 December 2013

Les interférons (IFN) constituent une famille de cytokines aux propriétés antiprolifératives et antivirales. Ils activent, via la voie Jak/STAT, des gènes spécifiques dont les produits sont les médiateurs des effets biologiques des IFN. C’est le cas de PML (Promyelocytic leukemia), appelée aussi TRIM19, qui joue un rôle central dans la défense antivirale. PML appartenant à la famille des protéines Tripartite Motif (TRIM), caractérisée par la présence en N-terminal d’un motif RBCC, constitué d’un domaine RING, d’une ou de deux boites B et d’un domaine coiled-coil. PML a été identifiée dans la leucémie aiguë promyélocytaire, une pathologie causée par la translocation chromosomique t(15 ;17) qui fusionne les gènes PML et RARA, aboutissant à la synthèse d'une protéine chimère PML-RARA. Le trioxyde d'arsenic (As2O3) cible la portion PML de la protéine oncogénique, entraînant sa dégradation et la rémission complète des patients. Dans les cellules saines, les transcrits PML issus d’un gène unique génèrent par épissage alternatif 7 isoformes principales de PML, dont six sont nucléaires (PMLI à PMLVI) et une cytoplasmique (PMLVIIb). Toutes possèdent la même extrémité N-terminale mais diffèrent au niveau de leur extrémité C-terminale, conférant à chaque isoforme des fonctions spécifiques.PML est l’organisatrice d’une structure multi-protéique appelée corps nucléaires (CN), impliquée dans divers processus cellulaires tels que l’apoptose, la dégradation des protéines ou encore la défense antivirale.PML est modifiée par SUMO de façon covalente au niveau de trois sites lysines (K65, K160, K490) et de façon non covalente, via son domaine SIM (pour « SUMO Interacting Motif »). Ces modifications sont requises pour la formation de CN fonctionnels et le recrutement de protéines partenaires au sein de ceux-ci. Le but de ma thèse a été d’étudier le rôle différentiel des différentes isoformes de PML en réponse à l’As2O3 et suite à l’infection virale. Nous avons montré que le SIM de PML est nécessaire à sa dégradation en réponse à l'As2O3. Ce motif est présent dans toutes les isoformes de PML, hormis l’isoforme nucléaire PMLVI et l’isoforme cytoplasmique PMLVIIb. Le SIM de PML n’est pas requis pour sa SUMOylation et son interaction avec RNF4 (une E3 ubiquitine ligase responsable de la dégradation de PML via le protéasome). En revanche, ce motif est requis pour l’ubiquitination de PML, le recrutement des composants du protéasome et sa dégradation en réponse à l’As2O3. Concernant les propriétés antivirales de PML, l’étude que nous avons menée avec toutes les isoformes de PML a permis de montrer que seules PMLIII et PMLIV confèrent une résistance au Virus de la Stomatite Vésiculaire (VSV). L’effet antiviral de PMLIII n'est observé qu'à faible multiplicité d’infection (MOI) et est indépendant de la production d’IFN. Par contre, PMLIV exerce une puissante activité anti-VSV, y compris à forte MOI et s'exerce selon deux mécanismes distincts : (i) PMLIV inhibe la réplication du VSV par un mécanisme précoce indépendant de l’IFN, (ii) PMLIV augmente tardivement la production d’IFN-β via une plus forte activation d’IRF3 qui est due à la séquestration spécifique de Pin1 au sein des CN par PMLIV. Ces deux processus nécessitent la SUMOylation de PMLIV. Ces résultats montrent que PMLIV exerce une activité antivirale intrinsèque et est impliquée dans l’immunité innée en régulant positivement la voie de transduction conduisant à la synthèse d’IFN-β. / Interferons (IFNs) are a family of cytokines with antiproliferative and antiviral properties.They activate, via the Jak/Stat pathway, specific genes whose products are the mediators of the biological effects of IFNs. This is the case of PML (Promyelocytic leukemia), also known as TRIM19, which plays a central role in antiviral defense.PML belongs to the Tripartite Motif (TRIM) protein family, characterized by the presence of an N- terminal RBCC pattern, consisting of a RING domain, one or two B-boxes and a coiled-coil domain. PML was identified in acute promyelocytic leukemia, a disease caused by the chromosomal translocation t(15 ;17), which fuses the PML and RARA genes, leading to the synthesis of a chimeric protein PML-RARA . Arsenic trioxide (As2O3) targets the PML moiety of the oncogenic protein, resulting in its degradation and in the complete remission of patients.In healthy cells, PML transcripts derived from a single gene generate seven major isoforms of PML by alternative splicing, including six nuclear (PMLI to PMLVI) and one cytoplasmic (PMLVIIb). All share the same N-terminus but differ at their C-terminus, giving each isoform specific functions.PML is the organizer of a multi-protein structure called nuclear bodies (NBs) that are involved in various cellular processes such as apoptosis, protein degradation or antiviral defense.PML is covalently modified by SUMO at three lysine residues (K65, K160, K490) but also non-covalently via its SIM domain (for « SUMO Interacting Motif »). These modifications are required for the formation of functional NBs and the recruitment of partner proteins within them.The aim of my thesis was to study the differential role of the different PML isoforms in response to As2O3 and during viral infection.We have shown that the SIM PML SIM is necessary for its degradation in response to As2O3. This motif is present in all PML isoforms, except the nuclear PMLVI and the cytoplasmic PMLVIIb isoforms. The SIM of PML is not required for its SUMOylation and its interaction with RNF4 (the E3 ubiquitin ligase responsible for PML proteasome-dependent degradation). However, this motif is required for the ubiquitination of PML, the recruitment of proteasome components and the degradation of PML in response to As2O3.Concerning the antiviral properties of PML, the study that we conducted with all PML isoforms allowed us to show that only PMLIII and PMLIV confer resistance to Vesicular Stomatitis Virus (VSV). Whereas the antiviral activity of PMLIII is only observed at low multiplicity of infection (MOI) and is independent of IFN production, PMLIV has a potent anti-VSV activity, including at high MOI, which is mediated through two distinct mechanisms: (i) PMLIV inhibits the replication of VSV by an early and IFN-independent mechanism, (ii) PMLIV later increases the production of IFN-β via a stronger activation of IRF3, which is due to the specific sequestration of Pin1 by PMLIV within NBs. Both processes require the PMLIV SUMOylation. These results show that PMLIV has an intrinsic antiviral activity and is also involved in innate immunity by positively regulating the transduction pathway leading to IFN-β synthesis.

PML/TRIM19

IFN-β

IRF3

Immunité innée

Immunité intrinsèque

Défense antivirale

Arsenic

Pin1

SUMO

SIM

VSV

PML/TRIM19

IFN-β

IRF3

Innate immunity

Intrinsic immunity

Antiviral defense

Arsenic

Pin1

SUMO

SIM

VSV

Etude des interactions entre la peptidyl-prolyl cis/trans isomérase Pin1 et la protéine microtubulaire Tau. Recherche d'inhibiteurs ciblant la liaison de Pin1 à ses substrats phosphorylés

Smet-Nocca, Caroline

18 October 2004

La phosphorylation constitue un mécanisme de régulation de la fonction biologique des protéines lié au contrôle des associations inter-moléculaires, de l'activité enzymatique ou de la liaison de ligands. L'isomérisation des liaisons Ser/Thr-Pro après phosphorylation par des kinases spécifiques, souvent impliquées dans le contrôle du cycle cellulaire, se présente comme un nouveau mode de régulation. Ces deux mécanismes de signalisation sont étroitement liés par l'intermédiaire d'enzymes catalysant l'isomérisation cis/trans des prolines au niveau de motifs Ser/Thr-Pro phosphorylés telles que les peptidyl-prolyl cis/trans isomérases de la famille de Pin1. Elles jouent un rôle cellulaire essentiel mais leur rôle moléculaire exact est encore mal connu. Les interactions moléculaires entre Pin1 et de nombreuses phospho-protéines mitotiques indiquent un rôle dans la régulation du cycle cellulaire et dans l'oncogénèse, et font de Pin1 une cible pharmacologique émergente dans le traitement des cancers. Récemment, des interactions avec la protéine microtubulaire Tau dans sa forme pathologique hyperphosphorylée, au niveau d'un site unique centré autour du motif Thr231-Pro232, pourraient impliquer Pin1 dans la régulation de la liaison de Tau aux microtubules et dans les phénomènes de neurodégénérescence observés dans la maladie d'Alzheimer.<br /><br />Nous avons ciblé les interactions entre Pin1 et la protéine Tau comme modèle de substrats pour une étude détaillée des mécanismes intervenant à l'échelle moléculaire, sur base de substrats peptidiques, qui permettraient d'expliquer le rôle fonctionnel de Pin1. L'interaction avec les substrats au travers des motifs Ser/Thr-Pro phosphorylés est double : un domaine de liaison WW permet la liaison du substrat et un domaine catalytique PPIase (peptidyl-prolyl isomérase) catalyse l'isomérisation cis/trans des prolines. Un criblage par RMN des différents motifs phospho-Ser/Thr-Pro au sein de la protéine Tau a permis de déterminer un nouveau site d'interaction centré autour du motif Thr212-Pro213, phosphorylé uniquement dans la forme pathologique de Tau. <br /><br />Nous avons étendu l'investigation des interactions avec Pin1 à l'échelle de la protéine Tau entière. Comme pour la plupart des régions protéiques impliquées dans les interactions avec Pin1, la protéine Tau se caractérise par une absence de structure globale qui limite considérablement les études par RMN. Un fragment peptidique de 40 acides aminés comprenant les sites Thr231 et Thr212 phosphorylés a permis de montrer un rôle régulateur du domaine WW dans l'activité enzymatique. Une première étude avec une protéine mutante mimant l'état phosphorylé de Tau a montré une interaction avec le domaine catalytique de Pin1 et a nécessité la mise au point préalable d'une technique d'attribution de la protéine Tau par RMN que nous avons appelé « mapping peptidique ».<br /><br />La phosphorylation du domaine WW de Pin1 est associée à l'inhibition de la liaison des substrats et joue un rôle dans la régulation de l'activité de Pin1 in vivo. La forme non phosphorylée active de Pin1 est retrouvée majoritairement dans les cellules cancéreuses et la forme phosphorylée inactive dans les cellules saines. Nous avons envisagé de cibler les interactions entre Pin1 et les phospho-peptides avec la synthèse de molécules organiques mimant le dipeptide phosphoThr-Pro et la mise en œuvre d'un test de criblage par RMN pour l'obtention d'inhibiteurs ciblant le domaine WW de Pin1 qui pourraient mimer la forme inactive de la protéine.

Spectroscopie RMN

peptidyl-prolyl cis/trans isomérase

Pin1

protéine Tau

interactions biomoléculaires

criblage

Progress of Weak Affinity Chromatography as a Tool in Drug Development

Meiby, Elinor

January 2013

Weak Affinity Chromatography (WAC) is a technology that was developed to analyse weak (KD &gt; 10-5 M) although selective interactions between biomolecules. The focus of this thesis was to develop this method for various applications in the drug development process.   Fragment Based Drug Discovery is a new approach in finding new small molecular drugs. Here, relatively small libraries (a few hundreds to a few thousands of compounds) of fragments (150 – 300 Da) are screened against the target. Fragment hits are then developed into lead molecules by linking, growing or merging fragments binding to different locations of the protein’s active site. However, due to the weakly binding nature of fragments, methods that are able to detect very weak binding events are needed. In this thesis, WAC is presented as a new robust and highly reproducible technology for fragment screening. The technology is demonstrated against a number of different protein targets – proteases, kinases, chaperones and protein-protein interaction (PPI) targets. Comparison of data from fragment screening of 111 fragments by WAC and other more established technologies for fragment screening, such as surface plasmon resonance (SPR) and nuclear magnetic resonance (NMR), validates WAC as a screening technology. It also points at the importance of performing fragment screening by multiple methods as they complement each other.   Other applications of WAC in drug development are also presented. The method can be used for chiral separations of racemic mixtures during fragment screening, which enables affinity measurements of individual enantiomers binding to the target of interest. Further, analysis of crude reaction mixtures is shown. By these procedures, the affinity of the product can be assessed directly after synthesis without any time-consuming purification steps. In addition, a high performance liquid chromatography (HPLC) system for highly efficient drug partition studies was developed by stable immobilization of lipid bilayer disks – lipodisks – on a high performance silica support material. These lipodisks are recognized model membranes for drug partition studies. A WAC system with incorporated membrane proteins into immobilized lipodisks has also been produced and evaluated with the ultimate objective to study affinity interactions between ligands and membrane proteins. / Ett läkemedel utövar sin funktion genom att påverka aktiviteten hos ett protein i kroppen då det binder till dess aktiva säte. Förändringen i aktivitet leder till fysiologiska förändringar i kroppen beroende på vilken funktion proteinet har. Med läkemedelsmolekyl avses här en liten organisk molekyl. Fragment-baserad läkemedelsutveckling är en ny metod for att ta fram nya läkemedel. Metoden fungerar genom att man bygger läkemedelsmolekyler utifrån mindre fragment som binder till målproteinet. Fragmenten hittar man genom att screena hela bibliotek av olika fragment mot samma målprotein för att urskilja de som binder till proteinets aktiva säte. Fördelen med den här metoden är bl. a. att med mindre molekyler som utgångspunkt kan en större del av antalet möjliga kombinationer av atomer representeras med ett mindre antal fragment än för större molekyler. Normalt utgörs ett fragmentbibliotek enbart av några hundra till några tusen substanser. Eftersom fragmenten är små har de få interaktionspunker och binder relativt svagt. De svaga bindningarna är svåra att se och mycket känsliga metoder behövs.   Svagaffinitetskromatografi är en vätskekromatografisk metod som utvecklades för att studera svaga men mycket selektiva bindningar mellan biomolekyler. Den här avhandlingen syftar till att utveckla metoden för olika användningsområden inom läkemedelsutveckling, främst som en ny metod för fragment-screening. Här mäter man interaktionen mellan ett protein och ett fragment. Proteinet kopplas till ett material som sedan packas i en kolonn i formen av en cylinder. När provet pumpas igenom kolonnen kommer de analyter med affinitet till proteinets aktiva säte att fördröjas på kolonnen i relation till hur starkt de interagerar med målproteinet.   I den här avhandlingen presenteras fragment-screening med svagaffinitetskromatografi gentemot ett antal olika typer av målproteiner. Resultatet överensstämmer väl med andra metoder för fragment-screening. Analys av reaktionsblandningar med svagaffinitetskromatografi demonstreras också. Därmed kan bindningen mellan en produkt i en reaktionsblandning och ett målprotein mätas direkt utan föregående uppreningssteg av reaktionsblandningen. Lipodiskar är små diskformade modellmembran som kan användas för att bl. a. mäta hur effektivt läkemedlet tas upp i kroppen vid behandling. Ett system med immobiliserade lipodiskar i en kolonn utvecklades med det framtida målet att kunna arbeta med membranproteiner med svagaffinitetskromatografi.   Detta arbete utgör en del i att utveckla svagaffinitetskromatografi som en lättillgänglig och relativt billig metod för användning inom industrin och akademin för läkemedelsutveckling.

weak affinity chromatography

fragment based drug discovery

fragment screening

thrombin

trypsin

cyclin G-associated kinase

Hsp90

Pin1

cyclooxygenase

lipodisks

Molecular Dynamics Simulations Towards The Understanding of the Cis-Trans Isomerization of Proline As A Conformational Switch For The Regulation of Biological Processes

Velazquez, Hector

10 May 2014

Pin1 is an enzyme central to cell signaling pathways because it catalyzes the cis–trans isomerization of the peptide ω-bond in phosphorylated serine/threonine-proline motifs in many proteins. This regulatory function makes Pin1 a drug target in the treatment of various diseases. The effects of phosphorylation on Pin1 substrates and the basis for Pin1 recognition are not well understood. The conformational consequences of phosphorylation on Pin1 substrate analogues and the mechanism of recognition by the catalytic domain of Pin1 were determined using molecular dynamics simulations. Phosphorylation perturbs the backbone conformational space of Pin1 substrate analogues. It is also shown that Pin1 recognizes specific conformations of its substrate by conformational selection. Dynamical correlated motions in the free Pin1 enzyme are present in the enzyme of the enzyme–substrate complex when the substrate is in the transition state configuration. This suggests that these motions play a significant role during catalysis. These results provide a detailed mechanistic understanding of Pin1 substrate recognition that can be exploited for drug design purposes and further our understanding of the subtleties of post-translational phosphorylation and cis–trans isomerization. Results from accelerated molecular dynamics simulations indicate that catalysis occurs along a restricted path of the backbone configuration of the substrate, selecting specific subpopulations of the conformational space of the substrate in the active site of Pin1. The simulations show that the enzyme–substrate interactions are coupled to the state of the prolyl peptide bond during catalysis. The transition-state configuration of the substrate binds better than the cis and trans states to the catalytic domain of Pin1. This suggests that Pin1 catalyzes its substrate by noncovalently stabilizing the transition state. These results suggest an atomistic detail understanding of the catalytic mechanism of Pin1 that is necessary for the design of novel inhibitors and the treatment of several diseases. Additionally, a set of constant force biased molecular dynamics simulations are presented to explore the kinetic properties of a Pin1 substrate and its unphosphorylated analogue. The simulations indicate that the phosphorylated Pin1 substrate isomerizes slower than the unphosphorylated analogue. This is due to the lower diffusion constant for the phosphorylated Pin1 substrate.

Pin1

Accelerated molecular dynamics

Cis-trans isomerization

PPIases

Enzyme dynamics

Peptidyl-prolyl cis-trans isomerase

Molecular switches

Protein regulation

Regulation of tumor growth by synthetic disintegrins or depletion of PIN1

Schneider, Ryan Anthony

17 December 2010

No description available.

Molecular Biology

Oncology

Pharmaceuticals

Pharmacology

Pharmacy Sciences

Cancer

integrin

disintegrin

PIN1

proline-isomerase

VEGF

HIF-1alpha

caspase-3

Design, Syntheses, and Bioactivities of Conformationally Locked Pin1 Ground State Inhibitors

Wang, Xiaodong

12 April 2005

Pin1 (protein interacting with NIMA 1) is a peptidyl-prolyl isomerase involved in mitosis. As a potential anti-cancer drug target, Pin1 interacts and regulates the activity of an increasing number of cell cycle enzymes by an unknown mechanism. These cell cycle enzymes include Cdc25, Cdc27, Cyclin D1, Myt1, Wee1, NIMA, Cdc2, Plk1 and c-Myc. Recent research has revealed that Pin1 is overexpressed in a variety of cancer cell lines and Pin1 inhibitors inhibit proliferation activity of several cancer cells overexpressing Pin1. The most potent Pin1 inhibitors identified so far are in the micromolar range and no pharmacophore has been identified. In order to assist the understanding of the biological function of Pin1 using molecular probes, two amide isosteres of Ser-<i>trans</i>-Pro and Ser-<i>cis</i>-Pro dipeptides were designed and stereoselectively synthesized. The conformationally locked Ser–<i>trans</i>–Pro mimic, Boc-SerΨ[(<i>E</i>)CH=C]Pro–OH, was synthesized through the use of an Ireland-Claisen [3,3]-sigmatropic rearrangement in nine steps with 13% overall yield from a serine derivative. The Ser-<i>cis</i>-Pro mimic, Boc-SerΨ[(<i>Z</i>)CH=C]Pro–OH, was synthesized through the use of a Still-Wittig [2,3]-sigmatropic rearrangement in 11 steps with an overall yield of 20% from the same starting material. Conformationally locked peptidomimetics, including two exactly matched peptidomimetics, Ac–Phe–Phe–pSer–Ψ(<i>E</i>)CH=C]Pro–Arg–NH2 and Ac–Phe–Phe–pSer–Ψ[(<i>Z</i>)CH=C]Pro–Arg–NH2, were synthesized from these Ser-Pro isosteres using Fmoc SPPS. A protocol for in vitro Pin1 inhibition assay was established for measuring the inhibition constant for these peptidomimetics. A conformationally locked cis peptidomimetic inhibits Pin1 with a <i>K</i>_i of 1.7 <i>μ</i>M, 23-fold more potent than its trans counterpart, illustrating the preference of Pin1 for a cis amide bond in its PPIase domain. The A2780 ovarian cancer cell antiproliferation activity of these peptidomimetics parallels their respective Pin1 inhibition data. This research provides a start toward more drug-like Pin1 inhibitor design. Gly–<i>trans</i>–Pro isosteres were synthesized using the Ireland-Claisen route. The construction of a non-peptidic (Z)-alkene library for Pin1 inhibition was attempted using the Ser-<i>cis</i>-Pro mimic, Boc—SerΨ[(Z)CH=C]Pro–OH as the core. / Ph. D.

conformation

collagen

inhibition

assay

Ser-trans-Pro

Ser-cis-Pro

peptidomimetics

solid phase peptide synthesis

cell cycle

Pin1

isosteres

mimic

Recombinant Proteins for Biomedical Applications

Kim, Christina Sue Kyung

06 July 2020

Both technological and experimental advancements in the field of biotechnology have allowed scientists to make leaps in areas such nucleic acid, antibody, and recombinant protein technologies. Here we focus on the use of recombinant proteins as molecular recognition motifs, wound healing biomaterials, and agents for cell cycle pathway elucidation are discussed. The author's primary project is described in chapters 2 and 3, and is focused on designed leucine-rich repeat proteins which offer increased stability, modularity, and surface area for binding interactions. These proteins bind at least two muramyl dipeptide ligands with picomolar to nanomolar affinity (Kd1 = 0.04 – 3.5 nM); as measured by fluorescence quenching experiments and ITC. The longest designed repeat, CLRR8, has a Kd app value of 1.0 nM which is comparable to full length native NOD2 protein. Molecular docking simulations revealed the locations of two potential binding sites and their respective interactions. The series of proteins represents a foundation for a high affinity and highly specific molecular recognition scaffold that has the potential to bind a variety of ligands. Previously the author contributed to the design of recombinant keratin proteins, and the work in Chapter 4 builds on the original design to allow for controlled degradation in wound healing systems. Site-directed mutagenesis was utilized to introduce these degradation sites, and modified keratin proteins were expressed with no differences to native recombinant keratin proteins. Success in engineering a variation of native keratin protein with no issues in expression lay the foundation for further engineering of native keratin or other relevant proteins for improved functionality. Chapter 5 describes steps towards producing human Aurora borealis (Bora) protein, an important substrate in cell cycle regulation, by in vitro transcription-translation with locked Ser–Pro analogues. This will allow for the elucidation of the active isomerization form to ensure proper cell division. Site-directed mutagenesis successfully introduced the amber codon to relevant Ser-Pro sites at positions 274 and 278. These mutated Bora genes along with modified ribosomes and aminoacyl tRNA will allow for the incorporation of locked dipeptide analogues. Expression of native Bora was carried out as a control, and appeared to express in dimeric form. The experiments carried out in Chapter 5 describe and outline all the molecular biology work completed and to be completed for this novel method of studying cis-trans isomerization in living cells. / Doctor of Philosophy / Sequencing of the human genome and the rapid development of gene editing and recombinant DNA technologies paved the way for a massive shift in the pharmaceutical industry. The first pharmaceutical companies in the 19th century started as fine chemicals businesses. The discovery of penicillin introduced antibiotics, and improved synthetic techniques led to the giants we know as big pharma today. Today, in the 21st century both computing and biotechnology has allowed for great leaps forward in precision medicine. Biotechnology refers to the manipulation of living organisms or their components to produce useful commercial products. In the pharmaceutical industry this refers to genetic engineering for novel pharmaceuticals. Here, we focus on the use of recombinant technology to create proteins for use in biomedical applications. Recombinant proteins are proteins formed by laboratory methods of molecular cloning. Through this technology, we are able to elucidate sequence-structure-function relationships of proteins, and determine their specific functions. Additionally, recombinant methods allow us to fine tune or modify the sequences of natural proteins to be more effective scaffolds or reagents. Chapter 3 focuses on the development of synthetic proteins for medical diagnostics. We designed a protein scaffold, based on natural innate immunity proteins, to detect bacteria cell wall components. Chapter 4 focuses on the engineering of keratin protein with applications in wound healing. We introduce controlled degradation of the biomaterial for use in potential drug delivery systems at the wound site. Chapter 5 focuses on the use of recombinant technologies aiding in the elucidation of a regulatory protein's function in cell division.

recombinant

protein engineering

consensus design

repeat proteins

LRR

molecular recognition motifs

keratin

biomaterials

Aurora A

Bora

Pin1

cell cycle

Pin1 Catalytic and WW Domain Ligands

Chen, Xingguo Ronald

10 June 2011

Pin1 is a peptidyl prolyl isomerase (PPIase) enzyme with two domains, the catalytic domain and the WW domain. Both domains specifically bind pSer/pThr–Pro motifs. Pin1 plays an important role in regulating the cell cycle, and it is involved in many diseases, such as cancer, HIV-1, Alzheimer's disease, asthma, hepatitis B, and rheumatoid arthritis. Pin1 is a very promising target for new drug development. Three stereoisomers: (R,S)-, (S,R)- and (S,S)-Ac–pSer–Ψ[(Z)CH=C]–Pip–2-(2-naphthyl)ethylamine were synthesized as inhibitors binding to the Pin1 catalytic domain. The (R,S)- and (S,R)-isomers were synthesized via a 13-step route, with overall yields of 2.0% and 1.4%, respectively. The newly formed stereogenic center in the piperidyl ring was introduced by a Luche reduction, followed by a stereoselective [2,3]-Still-Wittig rearrangement. The configuration of the stereocenter was determined by NOESY of a bicyclic derivative. The (Z)- to (E)-alkene ratio in the rearrangement was (5.5:1). The (S,S)-isomer was obtained as the epimerized by-product resulting from the (S,R)-isomer in the Na/NH3 deprotection step. The IC50 values for Pin1 inhibition were: 52, 85, and 141 μM, respectively. We concluded that in this Z-alkene isostere, the R-configuration would be preferred at both stereogenic centers, as mimics of L-Ser and L-Pip, to improve the affinity. Combinatorial chemistry is a powerful method to discover biologically active compounds, and solid-phase synthesis is most commonly used to synthesize combinatorial libraries. To identify ligands for the Pin1 WW domain, a library, R1CO–pSer–Pro–NHR2, was designed. A new solid-phase phosphorylating reagent (SPPR) containing a phosphoramidite function was synthesized in one step from commercially available Wang resin. The SPPR was applied in the preparation of a designed library through parallel synthesis. The library contained 357 members (17 Ã 21), and was screened by an enzyme-linked enzyme binding assay (ELEBA). The best hits were resynthesized, and the competitive dissociation constants, Kd-rel, were measured by ELEBA, with a Kd-rel value of 130 μM for the best ligand. The absolute dissociation constants will be measured by our collaborator, Prof. Jefferey Peng, University of Notre Dame, using NMR methods. Besides the identification of the Pin1 WW domain ligands, I created a practical method for solid-phase synthesis of phosphopeptides. / Ph. D.

Pin1

catalytic

WW domain

ligand

inhibition

mimic

conformation

phosphorylation

assay

ELEBA

combinatorial

library

solid-phase

synthesis

NMR

peptide

Development Of Cyclic Peptidyl Ligands Through A Combinatorial Library Approach

Liu, Tao

27 July 2011

No description available.

Biochemistry

Biomedical Research

Chemistry

Cyclic Peptides

Combinatorial Chemistry

One-Bead-One-Compound (OBOC) Library

Prolactin Recepotr

Pin1

HIV Capsid

Calcineurin

Cell Penetrating Peptide (CPP)

Part 1 Design, Synthesis and Bioactivity of a Phosphorylated Prodrug for the Inhibition of Pin1; Part 2 Conformational Specificity of Cdc25c Substrate for Cdc2 Kinase using LC-MS/MS

Zhao, Song

18 January 2008

The phosphorylation-dependent PPIase (peptidyl prolyl isomerase), Pin1 (Protein interacting with NIMA#1), has been found to regulate cell cycle through a simple conformational change, the cis-trans isomerization of phospho-Ser/Thr-Pro amide bonds. A variety of key cell cycle regulatory phosphoproteins, including Cdc25 phosphatase,Cdc27, p53 oncogene, c-Myc oncogene, Wee1 kinase, Myt1 kinase, and NIMA kinas, have been confirmed as substrates of Pin1. Pin1 was also observed to be overexpressed in a variety of cancer cell lines, and the inhibitors of Pin1 showed antiproliferative activities towards these cancer cells. These results implied that Pin1 might serve as a potential anti-cancer drug target. Besides, Pin1 has an important neuroprotective function and represents a potential new therapeutic agent for Alzheimer's disease. In order to understand the interaction between Pin1 and Cdc25c and the role of Pin1 in the mechanism for the regulation of mitosis, two amide isosteres, Ser-Ψ[(Z)CH=C]-Pro-OH and Ser-Ψ[(E)CH=C]-Pro-OH were incorporated into two peptidomimetics derived from human Cdc25c. Phosphorylation of these two peptidomimetics by the incubation with Cdc2 was studied using LC-MS/MS technique. It was found that Cdc2 kinase was conformationally specific to its Cdc25c substrate. Only the trans conformer of Cdc25c at its Ser168-Pro position can be recognized and phosphorylated by Cdc2 kinase, thereby creating the binding site for Pin1. In an effort to improve the cell permeability of the charged inhibitors of Pin1, bisPOM (pivaloyloxymethyl) prodrug moiety was introduced to mask the phosphate group of Fmoc-pSer-Ψ[(Z)CH=C]-Pro-(2)-N-(3)-ethylaminoindole, which is one inhibitor of Pin1. Fmoc-pSer-Ψ[(Z)CH=C]-Pro-(2)-N-(3)-ethylaminoindole and its bisPOM prodrug were synthesized efficiently starting with Boc-Ser-Ψ[(Z)CH=C]-Pro-OH in 24% and 12% yields respectively. The charged inhibitor showed a moderate inhibition towards Pin1 (IC50 = 28.3 μM). Its antiproliferative activity towards A2780 ovarian cancer cells (IC50 = 46.2 μM) was significantly improved by its bisPOM prodrug (IC50 = 26.9 μM), which is comparable to the IC50 of the charged inhibitor towards Pin1 enzymatic activity. These results not only established the bisPOM strategy as an efficient prodrug choice for Pin1 inhibitors, but also added additional evidence for Pin1 as a potential anticancer drug target. / Ph. D.

peptidomimetics

cell cycle

Cdc2

conformation

Cdc25

Ser-trans-Pro

Ser-cis-Pro

Pin1

isosteres

LC-MS/MS

assay

inhibition

kinase

phosphorylation