Your search keyword '"Gerardo Turcatti"' showing total 66 results

1. High-content, arrayed compound screens with rhinovirus, influenza A virus and herpes simplex virus infections

Author

Dominik Olszewski, Fanny Georgi, Luca Murer, Vardan Andriasyan, Fabien Kuttler, Anthony Petkidis, Robert Witte, Artur Yakimovich, Lucy Fischer, Alina Rozanova, Yohei Yamauchi, Gerardo Turcatti, and Urs F. Greber

Subjects

Science

Abstract

Measurement(s) transmission of virus • drug toxicity Technology Type(s) fluorescence microscopy Factor Type(s) virus genotype • cell line • incubation temperature • number of cells seeded/ seeding density • inoculation time • virus input FFU • drug concentration Sample Characteristic - Organism Homo sapiens • Rhinovirus A • Influenza A virus • Human alphaherpesvirus 1 Sample Characteristic - Environment epithelium Sample Characteristic - Location Switzerland

Published

2022

2. Synthesis and direct assay of large macrocycle diversities by combinatorial late-stage modification at picomole scale

Author

Sevan Habeshian, Manuel Leonardo Merz, Gontran Sangouard, Ganesh Kumar Mothukuri, Mischa Schüttel, Zsolt Bognár, Cristina Díaz-Perlas, Jonathan Vesin, Julien Bortoli Chapalay, Gerardo Turcatti, Laura Cendron, Alessandro Angelini, and Christian Heinis

Subjects

Science

Abstract

Macrocycles have potential as therapeutics, but their libraries are currently not large enough for high-throughput screening. Here, the authors show a combinatorial approach to generate a library of almost 20’000 macrocycles by conjugating carboxylic-acid fragments to macrocyclic scaffolds, identifying nanomolar inhibitors against thrombin and binders of MDM2.

Published

2022

3. Corrigendum: High-throughput, nonperturbing quantification of lipid droplets with digital holographic microscopy

Author

Vasco Campos, Benjamin Rappaz, Fabien Kuttler, Gerardo Turcatti, and Olaia Naveiras

Subjects

Biochemistry, QD415-436

Published

2022

4. Highly Potent Host-Specific Small-Molecule Inhibitor of Paramyxovirus and Pneumovirus Replication with High Resistance Barrier

Author

Neeta Shrestha, Flavio Max Gall, Cyrille Mathieu, Melanie Michaela Hierweger, Melanie Brügger, Marco P. Alves, Jonathan Vesin, Damiano Banfi, David Kalbermatter, Branka Horvat, Marc Chambon, Gerardo Turcatti, Dimitrios Fotiadis, Rainer Riedl, and Philippe Plattet

Subjects

paramyxovirus, pneumovirus, host-directed, replication, inhibitors, high resistance barrier, Microbiology, QR1-502

Abstract

ABSTRACT Multiple enveloped RNA viruses of the family Paramyxoviridae and Pneumoviridae, like measles virus (MeV), Nipah virus (NiV), canine distemper virus (CDV), or respiratory syncytial virus (RSV), are of high clinical relevance. Each year a huge number of lives are lost as a result of these viral infections. Worldwide, MeV infection alone is responsible for over a hundred thousand deaths each year despite available vaccine. Therefore, there is an urgent need for treatment options to counteract these viral infections. The development of antiviral drugs in general stands as a huge challenge due to the rapid emergence of viral escape mutants. Here, we disclose the discovery of a small-molecule antiviral, compound 1 (ZHAWOC9045), active against several pneumo-/paramyxoviruses, including MeV, NiV, CDV, RSV, and parainfluenza virus type 5 (PIV-5). A series of mechanistic characterizations revealed that compound 1 targets a host factor which is indispensable for viral genome replication. Drug resistance profiling against a paramyxovirus model (CDV) demonstrated no detectable adaptation despite prolonged time of investigation, thereby mitigating the rapid emergence of escape variants. Furthermore, a thorough structure-activity relationship analysis of compound 1 led to the invention of 100-times-more potent-derivatives, e.g., compound 2 (ZHAWOC21026). Collectively, we present in this study an attractive host-directed pneumoviral/paramyxoviral replication inhibitor with potential therapeutic application. IMPORTANCE Measles virus, respiratory syncytial virus, canine distemper virus, and Nipah virus are some of the clinically significant RNA viruses that threaten substantial number of lives each year. Limited to no availability of treatment options for these viral infections makes it arduous to handle the outbreaks. This highlights the major importance of developing antivirals to fight not only ongoing infections but also potential future epidemics. Most of the discovered antivirals, in clinical trials currently, are virus targeted, which consequently poses the challenge of rapid emergence of escape variants. Here, we present compound 1 (ZHAWOC9045), discovered to target viral replication in a host-dependent manner, thereby exhibiting broad-spectrum activity against several members of the family Pneumo-/Paramyxoviridae. The inability of viruses to mutate against the inhibitor mitigated the critical issue of generation of escape variants. Importantly, compound 1 was successfully optimized to a highly potent variant, compound 2 (ZHAWOC21026), with a promising profile for pharmacological intervention.

Published

2021

5. Loss of Bacterial Cell Pole Stabilization in Caulobacter crescentus Sensitizes to Outer Membrane Stress and Peptidoglycan-Directed Antibiotics

Author

Simon-Ulysse Vallet, Lykke Haastrup Hansen, Freja Cecillie Bistrup, Signe Aagaard Laursen, Julien Bortoli Chapalay, Marc Chambon, Gerardo Turcatti, Patrick H. Viollier, and Clare L. Kirkpatrick

Subjects

antibiotic resistance, Caulobacter crescentus, TonB-dependent receptor, cell envelope, cell polarity, vancomycin, Microbiology, QR1-502

Abstract

ABSTRACT Rod-shaped bacteria frequently localize proteins to one or both cell poles in order to regulate processes such as chromosome replication or polar organelle development. However, the roles of polar factors in responses to extracellular stimuli have been generally unexplored. We employed chemical-genetic screening to probe the interaction between one such factor from Caulobacter crescentus, TipN, and extracellular stress and found that TipN is required for normal resistance of cell envelope-directed antibiotics, including vancomycin which does not normally inhibit growth of Gram-negative bacteria. Forward genetic screening for suppressors of vancomycin sensitivity in the absence of TipN revealed the TonB-dependent receptor ChvT as the mediator of vancomycin sensitivity. Loss of ChvT improved resistance to vancomycin and cefixime in the otherwise sensitive ΔtipN strain. The activity of the two-component system regulating ChvT (ChvIG) was increased in ΔtipN cells relative to the wild type under some, but not all, cell wall stress conditions that this strain was sensitized to, in particular cefixime and detergent exposure. Together, these results indicate that TipN contributes to cell envelope stress resistance in addition to its roles in intracellular development, and its loss influences signaling through the ChvIG two-component system which has been co-opted as a sensor of cell wall stress in Caulobacter. IMPORTANCE Maintenance of an intact cell envelope is essential for free-living bacteria to protect themselves against their environment. In the case of rod-shaped bacteria, the poles of the cell are potential weak points in the cell envelope due to the high curvature of the layers and the need to break and reform the cell envelope at the division plane as the cells divide. We have found that TipN, a factor required for correct division and cell pole development in Caulobacter crescentus, is also needed for maintaining normal levels of resistance to cell wall-targeting antibiotics such as vancomycin and cefixime, which interfere with peptidoglycan synthesis. Since TipN is normally located at the poles of the cell and at the division plane just before cells complete division, our results suggest that it is involved in stabilization of these weak points of the cell envelope as well as its other roles inside the cell.

Published

2020

6. Novel High-Throughput Fluorescence-Based Assay for the Identification of Nematocidal Compounds That Target the Blood-Feeding Pathway

Author

Anthony Marchand, Joyce W. M. Van Bree, Aya C. Taki, Mati Moyat, Gerardo Turcatti, Marc Chambon, Adam Alexander Thil Smith, Rory Doolan, Robin B. Gasser, Nicola Laraine Harris, and Tiffany Bouchery

Subjects

drug-screening, helminth, hookworm, blood-feeding, viability, fluorescence, Medicine, Pharmacy and materia medica, RS1-441

Abstract

Hookworm infections cause a neglected tropical disease (NTD) affecting ~740 million people worldwide, principally those living in disadvantaged communities. Infections can cause high morbidity due to their impact on nutrient uptake and their need to feed on host blood, resulting in a loss of iron and protein, which can lead to severe anaemia and impaired cognitive development in children. Currently, only one drug, albendazole is efficient to treat hookworm infection and the scientific community fears the rise of resistant strains. As part of on-going efforts to control hookworm infections and its associated morbidities, new drugs are urgently needed. We focused on targeting the blood-feeding pathway, which is essential to the parasite survival and reproduction, using the laboratory hookworm model Nippostrongylus brasiliensis (a nematode of rodents with a similar life cycle to hookworms). We established an in vitro-drug screening assay based on a fluorescent-based measurement of parasite viability during blood-feeding to identify novel therapeutic targets. A first screen of a library of 2654 natural compounds identified four that caused decreased worm viability in a blood-feeding-dependent manner. This new screening assay has significant potential to accelerate the discovery of new drugs against hookworms.

Published

2022

7. Assay for high-throughput screening of inhibitors of the ASC-PYD inflammasome core filament

Author

Lorenzo Sborgi, Johanna Ude, Mathias S. Dick, Jonathan Vesin, Marc Chambon, Gerardo Turcatti, Petr Broz, and Sebastian Hiller

Subjects

high-throughput screening, polarization anisotropy assay, inflammasome, ASC, pyroptotic cell death, inflammation, Medicine, Biology (General), QH301-705.5

Abstract

The protein ASC is a central component of most inflammasome complexes, forming functional oligomeric filaments that activate large amounts of pro-caspase-1 for further IL-1β processing and the induction of Gasdermin D-dependent cell death. The central role of inflammasomes in the innate immune response pose them as new molecular targets for therapy of diverse acute, chronic and inherited autoinflammatory pathologies. In recent years, an increasing number of molecules were proposed to modulate inflammasome signalling by interacting with different components of inflammasome complexes. However, the difficult in vitro reconstitution of the inflammasome has limited the development of specific on-target biochemical assays for compound activity confirmation and for drug discovery in high throughput screening setups. Here we describe a homogeneous, pH-based ASC oligomerization assay that employs fluorescence anisotropy (FA) to monitor the in vitro filament formation of the PYD domain of human ASC. The absence of additional solubility tags as well as of proteolytic enzymes to initiate the filament reaction makes this assay suitable for testing the direct effect of small molecules on filament formation in high throughput format. The ability of the assay to detect modulators of filament formation was confirmed by using a non-filament forming PYD mutant. The high and reproducible Z’-factor of 0.7 allowed to screen 10,100 compounds by high-throughput screening (HTS) aiming to identify inhibitors of ASC filament. While none of these molecules was able to inhibit ASC filament formation in vitro, the assay is directly amenable to screen other compound classes or validate candidate molecules from other screens.

Published

2018

8. High-throughput, nonperturbing quantification of lipid droplets with digital holographic microscopy

Author

Vasco Campos, Benjamin Rappaz, Fabien Kuttler, Gerardo Turcatti, and Olaia Naveiras

Subjects

adipogenesis, adipocyte, label-free, Biochemistry, QD415-436

Abstract

In vitro differentiating adipocytes are sensitive to liquid manipulations and have the tendency to float. Assessing adipocyte differentiation using current microscopy techniques involves cell staining and washing, while using flow cytometry involves cell retrieval in suspension. These methods induce biases, are difficult to reproduce, and involve tedious optimizations. In this study, we present digital holographic microscopy (DHM) as a label-free, nonperturbing means to quantify lipid droplets in differentiating adipocytes in a robust medium- to high-throughput manner. Taking advantage of the high refractive index of lipid droplets, DHM can assess the production of intracellular lipid droplets by differences in phase shift in a quantitative manner. Adipocytic differentiation, combined with other morphological features including cell confluence and cell death, was tracked over 6 days in live OP9 mesenchymal stromal cells. We compared DHM with other currently available methods of lipid droplet quantification and demonstrated its robustness with modulators of adipocytic differentiation in a dose-responsive manner. This study suggests DHM as a novel marker-free nonperturbing method to study lipid droplet accumulation and may be envisioned for drug screens and mechanistic studies on adipocytic differentiation.

Published

2018

9. Antiviral Screen against Canine Distemper Virus-Induced Membrane Fusion Activity

Author

Neeta Shrestha, Flavio M. Gall, Jonathan Vesin, Marc Chambon, Gerardo Turcatti, Dimitrios Fotiadis, Rainer Riedl, and Philippe Plattet

Subjects

CDV, cell-based fusion assay, envelope glycoproteins, host cell receptor, inhibitor discovery, Microbiology, QR1-502

Abstract

Canine distemper virus (CDV), a close relative of the human pathogen measles virus (MeV), is an enveloped, negative sense RNA virus that belongs to the genus Morbillivirus and causes severe diseases in dogs and other carnivores. Although the vaccination is available as a preventive measure against the disease, the occasional vaccination failure highlights the importance of therapeutic alternatives such as antivirals against CDV. The morbilliviral cell entry system relies on two interacting envelope glycoproteins: the attachment (H) and fusion (F) proteins. Here, to potentially discover novel entry inhibitors targeting CDV H, F and/or the cognate receptor: signaling lymphocyte activation molecule (SLAM) proteins, we designed a quantitative cell-based fusion assay that matched high-throughput screening (HTS) settings. By screening two libraries of small molecule compounds, we successfully identified two membrane fusion inhibitors (F2736-3056 and F2261-0043). Although both inhibitors exhibited similarities in structure and potency with the small molecule compound 3G (an AS-48 class morbilliviral F-protein inhibitor), F2736-3056 displayed improved efficacy in blocking fusion activity when a 3G-escape variant was employed. Altogether, we present a cell-based fusion assay that can be utilized not only to discover antiviral agents against CDV but also to dissect the mechanism of morbilliviral-mediated cell-binding and cell-to-cell fusion activity.

Published

2021

10. Screening-based approach to discover effective platinum-based chemotherapies for cancers with poor prognosis.

Author

Hristo P Varbanov, Fabien Kuttler, Damiano Banfi, Gerardo Turcatti, and Paul J Dyson

Subjects

Medicine, Science

Abstract

Drug combinations are extensively used to treat cancer and are often selected according to complementary mechanisms. Here, we describe a cell-based high-throughput screening assay for identification of synergistic combinations between broadly applied platinum-based chemotherapeutics and drugs from a library composed of 1280 chemically and pharmacologically diverse (mostly FDA approved) compounds. The assay was performed on chemoresistant cell lines derived from lung (A549) and pancreatic (PANC-1) carcinoma, where platinum-based combination regimens are currently applied though with limited success. The synergistic combinations identified during the screening were validated by synergy quantification using the combination index method and via high content fluorescent microscopy analysis. New promising synergistic combinations discovered using this approach include compounds currently not used as anticancer drugs, such as cisplatin or carboplatin with hycanthone and cisplatin with spironolactone in pancreatic carcinoma, and carboplatin and deferoxamine in non-small cell lung cancer. Strong synergy between cisplatin or carboplatin and topotecan in PANC-1 cells, compared to A549 cells, suggests that this combination, currently used in lung cancer treatment regimens, could be applied to pancreatic carcinoma as well. Several drugs used to treat diseases other than cancer, including pyrvinium pamoate, auranofin, terfenadine and haloprogin, showed strong cytotoxicity on their own and synergistic interactions with platinum drugs. This study demonstrates that non-obvious drug combinations that would not be selected based on complementary mechanisms can be identified via high-throughput screening.

Published

2019

11. Repositioning approved drugs for the treatment of problematic cancers using a screening approach.

Author

Hristo P Varbanov, Fabien Kuttler, Damiano Banfi, Gerardo Turcatti, and Paul J Dyson

Subjects

Medicine, Science

Abstract

Advances in treatment strategies together with an earlier diagnosis have considerably increased the average survival of cancer patients over the last four decades. Nevertheless, despite the growing number of new antineoplastic agents introduced each year, there is still no adequate therapy for problematic malignancies such as pancreatic, lung and stomach cancers. Consequently, it is important to ensure that existing drugs used to treat other types of cancers, and potentially other diseases, are not overlooked when searching for new chemotherapy regimens for these problematic cancer types. We describe a screening approach that identifies chemotherapeutics for the treatment of lung and pancreatic cancers, based on drugs already approved for other applications. Initially, the 1280 chemically and pharmacologically diverse compounds from the Prestwick Chemical Library® (PCL) were screened against A549 (lung cancer) and PANC-1 (pancreatic carcinoma) cells using the PrestoBlue fluorescent-based cell viability assay. More than 100 compounds from the PCL were identified as hits in one or both cell lines (80 of them, being drugs used to treat diseases other than cancer). Selected PCL hits were further evaluated in a dose-response manner. Promising candidates for repositioning emanating from this study include antiparasitics, cardiac glycosides, as well as the anticancer drugs vorinostat and topotecan.

Published

2017

12. Chemical Biology Approaches to Membrane Homeostasis and Function

Author

Miwa Takahashi-Umebayashi, Kai Johnsson, Luc Reymond, Aurélien Roux, Robbie Loewith, Gerardo Turcatti, Christian Heinis, Stefan Matile, David Alonso Doval, Andreas Zumbuehl, Thomas Hannich, Ludovic Pineau, and Howard Riezman

Subjects

Chemical biology, Fluorescent dyes, Giant unilamellar vesicles, Insulin receptor, Membranes, Microdomains, Chemistry, QD1-999

Abstract

The study of membranes is at a turning point. New theories about membrane structure and function have recently been proposed, however, new technologies, combining chemical, physical, and biochemical approaches are necessary to test these hypotheses. In particular, the NCCR in chemical biology aims to visualize and characterize membrane microdomains and determine their function during hormone signaling.

Published

2011

13. Picomole‐Scale Synthesis and Screening of Macrocyclic Compound Libraries by Acoustic Liquid Transfer

Author

Gontran Sangouard, Alessandro Zorzi, Yuteng Wu, Edouard Ehret, Mischa Schüttel, Sangram Kale, Cristina Díaz‐Perlas, Jonathan Vesin, Julien Bortoli Chapalay, Gerardo Turcatti, and Christian Heinis

Subjects

Liquid transfer, Macrocyclic Compounds, Chemistry, Scale (chemistry), acoustic droplet ejection, droplet ejection, design, protein-protein interactions, Proto-Oncogene Proteins c-mdm2, Acoustics, General Medicine, General Chemistry, picomole scale, Combinatorial synthesis, Combinatorial chemistry, Catalysis, macrocycles, Reagent, Humans, Tumor Suppressor Protein p53, Acoustic droplet ejection, combinatorial synthesis, Protein Binding

Abstract

Macrocyclic compounds are an attractive class of therapeutic ligands against challenging targets, such as protein-protein interactions. However, the development of macrocycles as drugs is hindered by the lack of large combinatorial macrocyclic libraries, which are cumbersome, expensive, and time consuming to make, screen, and deconvolute. Here, we established a strategy for synthesizing and screening combinatorial libraries on a picomolar scale by using acoustic droplet ejection to combine building blocks at nanoliter volumes, which reduced the reaction volumes, reagent consumption, and synthesis time. As a proof-of-concept, we assembled a 2700-member target-focused macrocyclic library that we could subsequently assay in the same microtiter synthesis plates, saving the need for additional transfers and deconvolution schemes. We screened the library against the MDM2-p53 protein-protein interaction and generated micromolar and sub-micromolar inhibitors. Our approach based on acoustic liquid transfer provides a general strategy for the development of macrocycle ligands.

Published

2021

14. Macrocycle synthesis strategy based on step-wise 'adding and reacting' three components enables screening of large combinatorial libraries†

Author

Gerardo Turcatti, Julien Bortoli Chapalay, Alessandro Angelini, Kaycie Deyle, Sangram S. Kale, Jonathan Vesin, Alessandro Zorzi, Carl Leonard Stenbratt, Christian Heinis, Laura Cendron, and Ganesh Kumar Mothukuri

Subjects

Chemistry, Drug development, 010405 organic chemistry, Human plasma, Settore BIO/10 - Biochimica, General Chemistry, Tripeptide, Alkylation, 010402 general chemistry, 01 natural sciences, Combinatorial chemistry, 0104 chemical sciences

Abstract

Macrocycles provide an attractive modality for drug development, but generating ligands for new targets is hampered by the limited availability of large macrocycle libraries. We have established a solution-phase macrocycle synthesis strategy in which three building blocks are coupled sequentially in efficient alkylation reactions that eliminate the need for product purification. We demonstrate the power of the approach by combinatorially reacting 15 bromoacetamide-activated tripeptides, 42 amines, and 6 bis-electrophile cyclization linkers to generate a 3780-compound library with minimal effort. Screening against thrombin yielded a potent and selective inhibitor (Ki = 4.2 ± 0.8 nM) that efficiently blocked blood coagulation in human plasma. Structure–activity relationship and X-ray crystallography analysis revealed that two of the three building blocks acted synergistically and underscored the importance of combinatorial screening in macrocycle development. The three-component library synthesis approach is general and offers a promising avenue to generate macrocycle ligands to other targets., Combination of three efficient chemical reactions allows for solution-phase synthesis of 3780 macrocycles and identification of potent thrombin inhibitor.

Published

2020

15. Image-Based Marker-Free Screening of GABAA Agonists, Antagonists, and Modulators

Author

Benjamin Rappaz, Pierre Marquet, Damiano Banfi, Pascal Jourdain, Fabien Kuttler, and Gerardo Turcatti

Subjects

0303 health sciences, GABAA receptor, medicine.drug_class, business.industry, Pharmacology, 01 natural sciences, Biochemistry, Anxiolytic, 0104 chemical sciences, Analytical Chemistry, Hypnotic, 010404 medicinal & biomolecular chemistry, 03 medical and health sciences, nervous system, High-content screening, Chloride channel, medicine, Molecular Medicine, Ligand-gated ion channel, Receptor, business, 030304 developmental biology, Biotechnology, Ionotropic effect

Abstract

The ionotropic GABAA receptors represent the main target for different groups of widely used drugs having hypnotic and anxiolytic effects. So far, most approaches used to assess GABA activity invol...

Published

2020

16. In vitro-transfusional model for red-blood-cell study: the advantage of lowering hematocrit

Author

Emmanuel, Längst, David, Crettaz, Julien, Delobel, Raffaele, Renella, Manon, Bardyn, Gerardo, Turcatti, Jean-Daniel, Tissot, and Michel, Prudent

Abstract

The quality of red blood cells (RBCs) stored in red cell concentrates (RCCs) is influenced by processing, storage and donor characteristics, and can have a clinical impact on transfused patients. To evaluate RBC properties and their potential impact in a transfusion setting, a simple in vitro-transfusional model has been developed.Transfusion was simulated by mixing a washed RBC pool from two male-derived RCCs stored at 4°C with a pool of 15 male-derived fresh frozen plasma (FFP) units, representing the recipient, at a hematocrit (HCT) of 30% ("control" setting) or 5% (alternative model). The mixtures were incubated at 37°C, 5% of COThe 5%-HCT model restored the 2,3-DPG level and maintained the ATP level. Furthermore, glucose consumption and corresponding lactate production were increased in the 5%- vs the 30%-HCT condition. Lower hemolysis was observed with 5%-HCT, but only at day 2. However, morphological analysis by digital holographic microscopy (DHM) revealed a decreased fraction of discocytes at 5% rather than at 30% of HCT at storage day 2 but at day 43, the trend was inverted. Concordantly, RBCs incubated at 5% of HCT were more deformable than at 30% at day 43 (p0.0001).Higher metabolic activity of RBCs in the 5%-HCT condition was promoted by a higher glucose availability and limited cell-waste accumulation. The conditions of the new proposed model thus enabled rejuvenation of RBCs and maintained them in a physiological-close state in contrast to the 30%-HCT model. It may be used as a first approach to evaluate e.g., the impact of donor and recipient characteristics on RBC properties.

Published

2022

17. Abstract 3541: Tumoroid-based screening platform to test focal, chemo- and combination therapy for retinoblastoma

Author

Irina Sinenko, Fabien Kuttler, Valentin Simeonov, Alexandre Moulin, Christina Stathopoulos, Gerardo Turcatti, Adeline Berger, Francis Munier, and Paul Dyson

Subjects

Cancer Research, Oncology

Abstract

Current treatments for retinoblastoma, the most common intraocular malignancy, rely on a limited number of drugs repurposed from other pediatric cancer therapies. Drug toxicity and relapse of the disease necessitate new therapeutic strategies. The implementation of drug candidates in the clinic is usually followed by in vitro validation, which requires accurate and clinically relevant in vitro models. We report here a robust 3D tumoroid-based platform, for testing various clinical protocols, e.g. therapeutic agents following a single or repeated exposure, alone or in combination with focal therapy (thermotherapy). The platform, generated from the Y79 retinoblastoma cell line, consists of matrix-embedded tumoroids, which retain the key features of the disease and allow prolonged culture time. Following the optimization of growth conditions, the effect of single and repeated exposure to chemotherapeutic agents has been measured by high-throughput automated fluorescence imaging followed by quantification. The clinical conditions of chemothermotherapy have been recapitulated with a setup consisting of: an infrared diode laser (810 nm, 0.3 W) that heats the tumoroids in the presence of indocyanine green (50 µg/mL); a thermal camera to enable real-time temperature measurement; and an environment-controlled inverted microscope to ensure physiological conditions and precise focusing of the laser. Melphalan and carboplatin, two drugs currently used to treat retinoblastoma in clinical protocols of chemotherapy and chemothermotherapy respectively, have been applied to validate the system.Tumoroid viability and size progressively decreased over 4 weeks of repeated drug exposure with melphalan, reflecting the response of retinoblastoma in advanced clinical cases. Carboplatin treatment showed an activity enhancement in the tumoroid model similar to that observed in the clinic, when combined with focal therapy, demonstrating that the platform system closely recapitulates the clinical conditions. Inversely, the thermotherapy experimental protocol designed for 2D in vitro cell culture and commonly used to date, i.e. an incubation temperature increased to 42 °C for 1 h, did not show an improvement of the carboplatin cytotoxicity, confirming that our laser-based thermotherapy protocol provides a more accurate and clinically relevant drug response. Such an approach, combining physiologically relevant in vitro cancer models and investigation of drugs in well-established treatment modalities, can significantly reduce the number of new drug candidates that give false-positives or overestimated efficacies when evaluated in relevant in vivo models. It is expected that the platform will contribute to the implementation of new therapeutic strategies to treat retinoblastoma, and could also be adapted to other diseases for which repeated drug exposure and/or chemothermotherapy is relevant. Citation Format: Irina Sinenko, Fabien Kuttler, Valentin Simeonov, Alexandre Moulin, Christina Stathopoulos, Gerardo Turcatti, Adeline Berger, Francis Munier, Paul Dyson. Tumoroid-based screening platform to test focal, chemo- and combination therapy for retinoblastoma. [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2023; Part 1 (Regular and Invited Abstracts); 2023 Apr 14-19; Orlando, FL. Philadelphia (PA): AACR; Cancer Res 2023;83(7_Suppl):Abstract nr 3541.

Published

2023

18. Identification of broad anti-coronavirus chemical agents for repurposing against SARS-CoV-2 and variants of concern

Author

Daniela Sequeira, Liliane Yang, Gerardo Turcatti, Urs F. Greber, Alfonso Gomez-Gonzalez, Michael Bauer, Maarit Suomalainen, Fanny Georgi, Luca Murer, Dominik Olszewski, Vardan Andriasyan, Nicole Meili, Anthony Petkidis, Romain Volle, and Fabien Kuttler

Subjects

History, Posaconazole, Polymers and Plastics, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), viruses, Human coronavirus drug screen at single cell resolution in arrayed format, Infectious and parasitic diseases, RC109-216, medicine.disease_cause, Article, Industrial and Manufacturing Engineering, Human explant nasal and bronchial epithelial cells, medicine, Post-entry coronavirus inhibition, SARS-CoV-2 variants of concern, Mycophenolic acid, Business and International Management, Repurposing, Coronavirus, business.industry, Drug synergy in vitro, Ethics committee, virus diseases, General Medicine, Human airway, Repurposing methylene blue, Virology, Regimen, Chemical agents, business, medicine.drug

Abstract

Endemic human coronaviruses (hCoVs) 229E and OC43 cause respiratory disease with recurrent infections, while severe acute respiratory syndrome (SARS)-CoV-2 spreads across the world with impact on health and societies. Here, we report an image-based multicycle infection procedure with α-coronavirus hCoV-229E-eGFP in an arrayed chemical library screen of 5440 clinical and preclinical compounds. Toxicity counter selection and challenge with the β-coronaviruses OC43 and SARS-CoV-2 in tissue culture and human airway epithelial explant cultures (HAEEC) identified four FDA-approved compounds with oral availability. Methylene blue (MB, used for the treatment of methemoglobinemia), Mycophenolic acid (MPA, used in organ transplantation) and the anti-fungal agent Posaconazole (POS) had the broadest anti-CoV spectrum. They inhibited the shedding of SARS-CoV-2 and variants-of-concern (alpha, beta, gamma, delta) from HAEEC in either pre- or post exposure regimens at clinically relevant concentrations. Co-treatment of cultured cells with MB and the FDA-approved SARS-CoV-2 RNA-polymerase inhibitor Remdesivir reduced the effective anti-viral concentrations of MB by 2-fold, and Remdesivir by 4 to 10-fold, indicated by BLISS independence synergy modelling. Neither MB, nor MPA, nor POS affected the cell delivery of SARS-CoV-2 or OC43 (+)sense RNA, but blocked subsequent viral RNA accumulation in cells. Unlike Remdesivir, MB, MPA or POS did not reduce the release of viral RNA in post exposure regimen, thus indicating infection inhibition at a post-replicating step as well. In summary, the data emphasize the power of unbiased, full cycle compound screens to identify and repurpose broadly acting drugs against coronaviruses., Graphical abstract Image 1

Published

2022

19. Arrayed multicycle drug screens identify broadly acting chemical inhibitors for repurposing against SARS-CoV-2

Author

Nicole Meili, Maarit Suomalainen, Anthony Petkidis, Gerardo Turcatti, Liliane Yang, Daniela Sequeira, Dominik Olszewski, Urs F. Greber, Romain Volle, Fabien Kuttler, Luca Murer, Vardan Andriasyan, Michael Bauer, and Alfonso Gomez-Gonzalez

Subjects

business.industry, medicine.medical_treatment, virus diseases, medicine.disease_cause, Virology, Mycophenolic acid, Chemical library, Tissue culture, chemistry.chemical_compound, Cytokine, chemistry, Cell culture, Immunity, Toxicity, Medicine, business, Coronavirus, medicine.drug

Abstract

Coronaviruses (CoVs) circulate in humans and animals, and expand their host range by zoonotic and anthroponotic transmissions. Endemic human CoVs, such as 229E and OC43 cause limited respiratory disease, and elicit short term anti-viral immunity favoring recurrent infections. Yet, severe acute respir-atory syndrome (SARS)-CoV-2 spreads across the globe with unprecedented impact on societies and economics. The world lacks broadly effective and affordable anti-viral agents to fight the pandemic and reduce the death toll. Here, we developed an image-based multicycle replication assay for focus for-mation of α-coronavirus hCoV-229E-eGFP infected cells for screening with a chemical library of 5440 compounds arrayed in 384 well format. The library contained about 39% clinically used compounds, 26% in phase I, II or III clinical trials, and 34% in preclinical development. Hits were counter-selected against toxicity, and challenged with hCoV-OC43 and SARS-CoV-2 in tissue culture and human bronchial and nasal epithelial explant cultures from healthy donors. Fifty three compounds inhibited hCoV-229E-GFP, 39 of which at 50% effective concentrations (EC50) < 2μM, and were at least 2-fold separated from toxicity. Thirty nine of the 53 compounds inhibited the replication of hCoV-OC43, while SARS-CoV-2 was inhibited by 11 compounds in at least two of four tested cell lines. Six of the 11 compounds are FDA-approved, one of which is used in mouth wash formulations, and five are systemic and orally available. Here, we demonstrate that methylene blue (MB) and mycophenolic acid (MPA), two broadly available low cost compounds, strongly inhibited shedding of infectious SARS-CoV-2 at the apical side of the cultures, in either pre- or post-exposure regimens, with somewhat weaker effects on viral RNA release indicated by RT-qPCR measurements. Our study illustrates the power of full cycle screens in repurposing clinical compounds against SARS-CoV-2. Importantly, both MB and MPA reportedly act as immunosuppressants, making them interesting candidates to counteract the cytokine storms affecting COVID-19 patients.

Published

2021

20. Image- and Fluorescence-Based Test Shows Oxidant-Dependent Damages in Red Blood Cells and Enables Screening of Potential Protective Molecules

Author

Benjamin Rappaz, Gerardo Turcatti, Manon Bardyn, Jérôme Allard, Michel Prudent, Jean-Daniel Tissot, and David Crettaz

Subjects

Antioxidant, antioxidant, Erythrocytes, medicine.medical_treatment, red blood cell, digital holographic microscopy, 030204 cardiovascular system & hematology, Resveratrol, medicine.disease_cause, Antioxidants, Workflow, chemistry.chemical_compound, 0302 clinical medicine, Drug Discovery, Biology (General), oxidant, Spectroscopy, 0303 health sciences, General Medicine, Oxidants, Fluorescence, Computer Science Applications, Molecular Imaging, Chemistry, medicine.anatomical_structure, fluorescence, QH301-705.5, high-throughput screening, Article, Catalysis, Inorganic Chemistry, 03 medical and health sciences, medicine, Humans, Physical and Theoretical Chemistry, Molecular Biology, QD1-999, 030304 developmental biology, transfusion, Organic Chemistry, Ascorbic acid, High-Throughput Screening Assays, Red blood cell, Oxidative Stress, chemistry, Microscopy, Fluorescence, Biophysics, Uric acid, Trolox, Reactive Oxygen Species, Oxidative stress

Abstract

An increase of oxygen saturation within blood bags and metabolic dysregulation occur during storage of red blood cells (RBCs). It leads to the gradual exhaustion of RBC antioxidant protective system and, consequently, to a deleterious state of oxidative stress that plays a major role in the apparition of the so-called storage lesions. The present study describes the use of a test (called TSOX) based on fluorescence and label-free morphology readouts to simply and quickly evaluate the oxidant and antioxidant properties of various compounds in controlled conditions. Here, TSOX was applied to RBCs treated with four antioxidants (ascorbic acid, uric acid, trolox and resveratrol) and three oxidants (AAPH, diamide and H 2 O 2 ) at different concentrations. Two complementary readouts were chosen: first, where ROS generation was quantified using DCFH-DA fluorescent probe, and second, based on digital holographic microscopy that measures morphology alterations. All oxidants produced an increase of fluorescence, whereas H 2 O 2 did not visibly impact the RBC morphology. Significant protection was observed in three out of four of the added molecules. Of note, resveratrol induced diamond-shape "Tirocytes". The assay design was selected to be flexible, as well as compatible with high-throughput screening. In future experiments, the TSOX will serve to screen chemical libraries and probe molecules that could be added to the additive solution for RBCs storage.

Published

2021

21. Highly Potent Host-Specific Small-Molecule Inhibitor of Paramyxovirus and Pneumovirus Replication with High Resistance Barrier

Author

Gerardo Turcatti, Melanie Brügger, Neeta Shrestha, Marc Chambon, Melanie M. Hierweger, Jonathan Vesin, Branka Horvat, Cyrille Mathieu, Dimitrios Fotiadis, Flavio M. Gall, Philippe Plattet, Marco P. Alves, Rainer Riedl, Damiano Banfi, David Kalbermatter, Vetsuisse Faculty [Berne, Suisse], University of Bern, Zürich University of Applied Sciences (ZHAW), Centre International de Recherche en Infectiologie (CIRI), École normale supérieure de Lyon (ENS de Lyon)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Université Jean Monnet - Saint-Étienne (UJM)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), Institute of Virology and Immunology [Mittelhäusern] (IVI), Ecole Polytechnique Fédérale de Lausanne (EPFL), Centre International de Recherche en Infectiologie - UMR (CIRI), École normale supérieure - Lyon (ENS Lyon)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), and Mathieu, Cyrille

Subjects

viruses, [CHIM.THER]Chemical Sciences/Medicinal Chemistry, Virus Replication, 615: Pharmakologie und Therapeutik, drug-resistance, [SDV.MHEP.MI]Life Sciences [q-bio]/Human health and pathology/Infectious diseases, generation, Drug Discovery, inhibitors, Host factor, [SDV.MP.VIR] Life Sciences [q-bio]/Microbiology and Parasitology/Virology, 0303 health sciences, Paramyxoviridae Infections, 630 Agriculture, biology, QR1-502, 3. Good health, Paramyxoviridae, [SDV.MP.VIR]Life Sciences [q-bio]/Microbiology and Parasitology/Virology, [SDV.MHEP.MI] Life Sciences [q-bio]/Human health and pathology/Infectious diseases, entry, acid, Viral genome replication, Research Article, replication, Inhibitor, [CHIM.THER] Chemical Sciences/Medicinal Chemistry, 610 Medicine & health, rsv, Antiviral Agents, Microbiology, Virus, Measles virus, 03 medical and health sciences, host-directed, paramyxovirus, Virology, medicine, Humans, Pneumovirus Infections, pneumovirus, canine-distemper virus, 030304 developmental biology, 030306 microbiology, Canine distemper, high resistance barrier, medicine.disease, biology.organism_classification, Pneumoviridae, Viral replication, 579: Mikrobiologie, 570 Life sciences, rescue, protein

Abstract

Multiple enveloped RNA viruses of the family Paramyxoviridae and Pneumoviridae, like measles virus (MeV), Nipah virus (NiV), canine distemper virus (CDV), or respiratory syncytial virus (RSV), are of high clinical relevance. Each year a huge number of lives are lost as a result of these viral infections. Worldwide, MeV infection alone is responsible for over a hundred thousand deaths each year despite available vaccine. Therefore, there is an urgent need for treatment options to counteract these viral infections. The development of antiviral drugs in general stands as a huge challenge due to the rapid emergence of viral escape mutants. Here, we disclose the discovery of a small-molecule antiviral, compound 1 (ZHAWOC9045), active against several pneumo-/paramyxoviruses, including MeV, NiV, CDV, RSV, and parain-fluenza virus type 5 (PIV-5). A series of mechanistic characterizations revealed that compound 1 targets a host factor which is indispensable for viral genome replication. Drug resistance profiling against a paramyxovirus model (CDV) demonstrated no detectable adaptation despite prolonged time of investigation, thereby mitigating the rapid emergence of escape variants. Furthermore, a thorough structure-activity relationship analysis of compound 1 led to the invention of 100-times-more potent-derivatives, e.g., compound 2 (ZHAWOC21026). Collectively, we present in this study an attractive host-directed pneumoviral/paramyxoviral replication inhibitor with potential therapeutic application., IMPORTANCE Measles virus, respiratory syncytial virus, canine distemper virus, and Nipah virus are some of the clinically significant RNA viruses that threaten substantial number of lives each year. Limited to no availability of treatment options for these viral infections makes it arduous to handle the outbreaks. This highlights the major importance of developing antivirals to fight not only ongoing infections but also potential future epidemics. Most of the discovered antivirals, in clinical trials currently, are virus targeted, which consequently poses the challenge of rapid emergence of escape variants. Here, we present compound 1 (ZHAWOC9045), discovered to target viral replication in a host-dependent manner, thereby exhibiting broad-spectrum activity against several members of the family Pneumo-/Paramyxoviridae.

Published

2021

22. A high-content image-based drug screen of clinical compounds against cell transmission of adenovirus

Author

Urs F. Greber, Fabien Kuttler, Gerardo Turcatti, Artur Yakimovich, Robert Witte, Luca Murer, Fanny Georgi, Vardan Andriasyan, University of Zurich, and Greber, Urs F

Subjects

Data Descriptor, Drug Evaluation, Preclinical, Virus Replication, 1710 Information Systems, Chemical library, chemistry.chemical_compound, Adenovirus, 1804 Statistics, Probability and Uncertainty, 2613 Statistics and Probability, lcsh:Science, media_common, 0303 health sciences, Nelfinavir, Statistics, High-throughput screening, virus diseases, 10124 Institute of Molecular Life Sciences, Computer Science Applications, Statistics, Probability and Uncertainty, medicine.drug, 3304 Education, Information Systems, Drug, Statistics and Probability, media_common.quotation_subject, Drug development, Library and Information Sciences, Antiviral Agents, Education, Small Molecule Libraries, 03 medical and health sciences, Text mining, Viral entry, High-Throughput Screening Assays, medicine, 1706 Computer Science Applications, 030304 developmental biology, 030306 microbiology, business.industry, Adenoviruses, Human, Virology, Viral replication, chemistry, 570 Life sciences, biology, lcsh:Q, Probability and Uncertainty, 3309 Library and Information Sciences, business, Nelfinavir mesylate

Abstract

Human adenoviruses (HAdVs) are fatal to immuno-suppressed individuals, but no effective anti-HAdV therapy is available. Here, we present a novel image-based high-throughput screening (HTS) platform, which scores the full viral replication cycle from virus entry to dissemination of progeny and second-round infections. We analysed 1,280 small molecular weight compounds of the Prestwick Chemical Library (PCL) for interference with HAdV-C2 infection in a quadruplicate, blinded format, and performed robust image analyses and hit filtering. We present the entire set of the screening data including all images, image analyses and data processing pipelines. The data are made available at the Image Data Resource (IDR, idr0081). Our screen identified Nelfinavir mesylate as an inhibitor of HAdV-C2 multi-round plaque formation, but not single round infection. Nelfinavir has been FDA-approved for anti-retroviral therapy in humans. Our results underscore the power of image-based full cycle infection assays in identifying viral inhibitors with clinical potential., Measurement(s) nucleus • number of infected nuclei • infection index (number of infected nuclei/number of nuclei) • Plaque • fluorescent reporter intensity • percent cell viability Technology Type(s) epifluorescence microscopy • compound toxicity assay Factor Type(s) compound treatment Sample Characteristic - Organism Human mastadenovirus C Machine-accessible metadata file describing the reported data: 10.6084/m9.figshare.12594470

Published

2020

23. The FDA-approved drug Nelfinavir inhibits lytic cell-free transmission of human adenoviruses

Author

Nicole Meili, Fanny Georgi, Luca Murer, Urs F. Greber, Robert Witte, Lisa Yu, Gerardo Turcatti, Artur Yakimovich, Melanie Grove, Vardan Andriasyan, Silvio Hemmi, and Fabien Kuttler

Subjects

Lysis, biology, Chemistry, virus diseases, Adenovirus Death Protein, Virology, eye diseases, Virus, Nelfinavir, Lytic cycle, medicine, biology.protein, Antibody, medicine.drug, Proto-oncogene tyrosine-protein kinase Src, Nelfinavir mesylate

Abstract

Adenoviruses (AdVs) are prevalent and give rise to chronic and recurrent disease. The human AdV (HAdV) species B and C, such as HAdV-C2, C5 and B14, cause respiratory disease, and constitute a health threat for immuno-compromised individuals. HAdV-Cs are well known for lysing cells, owing to the E3 CR1-β-encoded adenovirus death protein (ADP). We previously reported a high-throughput image-based screening framework and identified an inhibitor of HAdV-C2 multi-round infection, Nelfinavir Mesylate. Nelfinavir is the active ingredient of Viracept, an FDA-approved inhibitor of the human immuno-deficiency virus (HIV) aspartyl protease, and used to treat acquired immunodeficiency syndrome (AIDS). It is not effective against single round HAdV infections. Here, we show that Nelfinavir inhibits the lytic cell-free transmission of HAdV, indicated by the suppression of comet-shaped infection foci in cell culture. Comet-shaped foci occur upon convection-based transmission of cell-free viral particles from an infected cell to neighbouring uninfected cells. HAdV lacking ADP was insensitive to Nelfinavir, but gave rise to comet-shaped foci indicating that ADP enhances but is not required for cell lysis. This was supported by the notion that HAdV-B14 and B14p1 lacking ADP were highly sensitive to Nelfinavir, although HAdV-A31, B3, B7, B11, B16, B21, D8, D30 or D37 were less sensitive. Conspicuously, Nelfinavir uncovered slow-growing round-shaped HAdV-C2 foci, independent of neutralizing antibodies in the medium, indicative of non-lytic cell-to-cell transmission. Our study demonstrates the repurposing potential of Nelfinavir with post-exposure efficacy against different HAdVs, and describes an alternative non-lytic cell-to-cell transmission mode of HAdV.Graphical AbstractFigure 1.

Published

2020

24. High-content image-based drug screen identifies a clinical compound against cell transmission of adenovirus

Author

Robert Witte, Fanny Georgi, Urs F. Greber, Artur Yakimovich, Vardan Andriasyan, Fabien Kuttler, Gerardo Turcatti, and Luca Murer

Subjects

Drug, Accession number (library science), business.industry, media_common.quotation_subject, virus diseases, medicine.disease, Virology, Chemical library, chemistry.chemical_compound, Nelfinavir, chemistry, Viral replication, Viral entry, medicine, Adenovirus infection, business, medicine.drug, media_common, Nelfinavir mesylate

Abstract

Human adenoviruses (HAdVs) are fatal to immuno-suppressed people, but no effective anti-HAdV therapy is available. Here, we present a novel image-based high-throughput screening (HTS) platform, which scores the full viral replication cycle from virus entry to dissemination of progeny. We analysed 1,280 small molecular weight compounds of the Prestwick Chemical Library (PCL) for interference with HAdV-C2 infection in a quadruplicate, blinded format, and included robust image analyses, and hit filtering. We present the entire set of the screening data including all the images, image analyses and data processing pipelines. The data are made available at the Image Data Repository (IDR) 1, accession number idr0081. Our screen identified Nelfinavir mesylate as an inhibitor of HAdV-C2 multi-round plaque formation, but not single round infection. Nelfinavir has been FDA-approved for anti-retroviral therapy in humans. Our results underscore the power of image-based full cycle infection assays in identifying viral inhibitors with clinical potential.

Published

2020

25. Identification of New Vulnerabilities in Conjunctival Melanoma Using Image-Based High Content Drug Screening

Author

Katya Nardou, Michael Nicolas, Fabien Kuttler, Katarina Cisarova, Elifnaz Celik, Mathieu Quinodoz, Nicolo Riggi, Olivier Michielin, Carlo Rivolta, Gerardo Turcatti, and Alexandre Pierre Moulin

Subjects

polo-like kinase, cyclin dependent kinase, Cancer Research, nras mutations, volasertib bi 6727, kinase 1, conjunctival melanoma, drug screening, kinase inhibitors, MAPK pathway, PI3K/mTOR pathway, aurora-kinase, Hsp90, Tirbanibulin, inhibitor dinaciclib mk-7965, dose-escalation, hsp90, mapk pathway, Oncology, antitumor-activity, mek inhibitor, 1st-in-human phase-i, pi3k, mtor pathway, tirbanibulin, braf

Abstract

Simple Summary We determined the sensitivity of several conjunctival melanoma cell lines to kinase inhibitors as well as a few other inhibitors using an image-based high throughput drug screening assay with 542 compounds. All cell lines demonstrated sensitivity to cell cycle inhibition, especially with polo-like inhibitors. The response to MAPK pathway inhibition was better in the presence of BRAF(V600E) mutations, while the response to PI3k/mTOR inhibition was better in the presence of the NRAS(Q61L) mutation. Our study uncovers a large panel of new vulnerabilities in conjunctival melanoma and establishes the background for the expansion of therapeutic options in the management of this tumor. Recent evidence suggests that numerous similarities exist between the genomic landscapes of both conjunctival and cutaneous melanoma. Since alterations of several components of the MAP kinases, PI3K/mTOR, and cell cycle pathways have been reported in conjunctival melanoma, we decided to assess the sensitivity of conjunctival melanoma to targeted inhibition mostly of kinase inhibitors. A high content drug screening assay based on automated fluorescence microscopy was performed in three conjunctival melanoma cell lines with different genomic backgrounds with 489 kinase inhibitors and 53 other inhibitors. IC50 and apoptosis induction were respectively assessed for 53 and 48 compounds. The genomic background influenced the response to MAK and PI3K/mTOR inhibition, more specifically cell lines with BRAF (V600E) mutations were more sensitive to BRAF/MEK inhibition, while CRMM2 bearing the NRAS(Q61L) mutation was more sensitive to PI3k/mTOR inhibition. All cell lines demonstrated sensitivity to cell cycle inhibition, being more pronounced in CRMM2, especially with polo-like inhibitors. Our data also revealed new vulnerabilities to Hsp90 and Src inhibition. This study demonstrates that the genomic background partially influences the response to targeted therapy and uncovers a large panel of potential vulnerabilities in conjunctival melanoma that may expand available options for the management of this tumor.

Published

2022

26. Targeting STING with covalent small-molecule inhibitors

Author

Andrea Ablasser, F. Gisou van der Goot, Simone M. Haag, Gerardo Turcatti, Muhammet F. Gulen, Rayk Behrendt, Laurence Abrami, Luc Reymond, Antoine Gibelin, Alexiane Decout, and Michael Heymann

Subjects

0301 basic medicine, Lipoylation, medicine.medical_treatment, Golgi Apparatus, Cell Line, Small Molecule Libraries, Mice, 03 medical and health sciences, symbols.namesake, 0302 clinical medicine, Palmitoylation, medicine, Animals, Humans, Cysteine, Binding Sites, Multidisciplinary, Innate immune system, Chemistry, Hereditary Autoinflammatory Diseases, Membrane Proteins, Golgi apparatus, Small molecule, eye diseases, Transmembrane protein, Cell biology, Mice, Inbred C57BL, Sting, 030104 developmental biology, Cytokine, 030220 oncology & carcinogenesis, Stimulator of interferon genes, symbols, Protein Binding, Signal Transduction

Abstract

Aberrant activation of innate immune pathways is associated with a variety of diseases. Progress in understanding the molecular mechanisms of innate immune pathways has led to the promise of targeted therapeutic approaches, but the development of drugs that act specifically on molecules of interest remains challenging. Here we report the discovery and characterization of highly potent and selective small-molecule antagonists of the stimulator of interferon genes (STING) protein, which is a central signalling component of the intracellular DNA sensing pathway1,2. Mechanistically, the identified compounds covalently target the predicted transmembrane cysteine residue 91 and thereby block the activation-induced palmitoylation of STING. Using these inhibitors, we show that the palmitoylation of STING is essential for its assembly into multimeric complexes at the Golgi apparatus and, in turn, for the recruitment of downstream signalling factors. The identified compounds and their derivatives reduce STING-mediated inflammatory cytokine production in both human and mouse cells. Furthermore, we show that these small-molecule antagonists attenuate pathological features of autoinflammatory disease in mice. In summary, our work uncovers a mechanism by which STING can be inhibited pharmacologically and demonstrates the potential of therapies that target STING for the treatment of autoinflammatory disease.

Published

2018

27. Assay for high-throughput screening of inhibitors of the ASC-PYD inflammasome core filament

Author

Marc Chambon, Lorenzo Sborgi, Petr Broz, Gerardo Turcatti, Johanna Ude, Sebastian Hiller, Mathias S. Dick, and Johnathan Vesin

Subjects

Cancer Research, Physiology, High-throughput screening, Mutant, lcsh:Medicine, ASC, Biochemistry, Genetics and Molecular Biology (miscellaneous), high-throughput screening, Protein filament, pyroptotic cell death, inflammasome, medicine, lcsh:QH301-705.5, Drug discovery, Chemistry, lcsh:R, Proteolytic enzymes, Inflammasome, Small molecule, In vitro, Cell biology, polarization anisotropy assay, lcsh:Biology (General), inflammation, Molecular Medicine, medicine.drug, Research Article

Abstract

The protein ASC is a central component of most inflammasome complexes, forming functional oligomeric filaments that activate large amounts of pro-caspase-1 for further IL-1β processing and the induction of Gasdermin D-dependent cell death. The central role of inflammasomes in the innate immune response pose them as new molecular targets for therapy of diverse acute, chronic and inherited autoinflammatory pathologies. In recent years, an increasing number of molecules were proposed to modulate inflammasome signalling by interacting with different components of inflammasome complexes. However, the difficult in vitro reconstitution of the inflammasome has limited the development of specific on-target biochemical assays for compound activity confirmation and for drug discovery in high throughput screening setups. Here we describe a homogeneous, pH-based ASC oligomerization assay that employs fluorescence anisotropy (FA) to monitor the in vitro filament formation of the PYD domain of human ASC. The absence of additional solubility tags as well as of proteolytic enzymes to initiate the filament reaction makes this assay suitable for testing the direct effect of small molecules on filament formation in high throughput format. The ability of the assay to detect modulators of filament formation was confirmed by using a non-filament forming PYD mutant. The high and reproducible Z'-factor of 0.7 allowed to screen 10,100 compounds by high-throughput screening (HTS) aiming to identify inhibitors of ASC filament. While none of these molecules was able to inhibit ASC filament formation in vitro, the assay is directly amenable to screen other compound classes or validate candidate molecules from other screens.

Published

2018

28. 2013 – A LABEL-FREE, HIGH-THROUGHPUT PHENOTYPIC SCREEN OF ADIPOCYTIC DIFFERENTIATION MODULATORS TO ACCELERATE HEMATOPOIETIC RECOVERY

Author

Olaia Naveiras, Frederica Schyrr, Vasco Campos, Alejandro Alonso-Calleja, Benoit von der Weid, Pernille Reiner, Vincent Gardeux, Rita Sarkis, Aurelien Oggier, Silvia Lopes, Damiano Banfi, Fabien Kuttler, Bart Deplancke, and Gerardo Turcatti

Subjects

Cancer Research, Genetics, Cell Biology, Hematology, Molecular Biology

Published

2022

29. High-throughput, nonperturbing quantification of lipid droplets with digital holographic microscopy

Author

Olaia Naveiras, Gerardo Turcatti, Benjamin Rappaz, Fabien Kuttler, and Vasco Campos

Subjects

0301 basic medicine, Cellular differentiation, Holography, QD415-436, adipocyte, label-free, Biochemistry, Cell Line, adipogenesis, Flow cytometry, Adipocytes/cytology, Adipocytes/metabolism, Cell Differentiation, Image Processing, Computer-Assisted, Lipid Droplets/metabolism, Microscopy, 03 medical and health sciences, Endocrinology, Lipid droplet, Methods, Adipocytes, medicine, Confluency, medicine.diagnostic_test, Chemistry, Lipid Droplets, Cell Biology, 030104 developmental biology, Adipogenesis, Biophysics, Digital holographic microscopy, Intracellular

Abstract

In vitro differentiating adipocytes are sensitive to liquid manipulations and have the tendency to float. Assessing adipocyte differentiation using current microscopy techniques involves cell staining and washing, while using flow cytometry involves cell retrieval in suspension. These methods induce biases, are difficult to reproduce, and involve tedious optimizations. In this study, we present digital holographic microscopy (DHM) as a label-free, nonperturbing means to quantify lipid droplets in differentiating adipocytes in a robust medium- to high-throughput manner. Taking advantage of the high refractive index of lipid droplets, DHM can assess the production of intracellular lipid droplets by differences in phase shift in a quantitative manner. Adipocytic differentiation, combined with other morphological features including cell confluence and cell death, was tracked over 6 days in live OP9 mesenchymal stromal cells. We compared DHM with other currently available methods of lipid droplet quantification and demonstrated its robustness with modulators of adipocytic differentiation in a dose-responsive manner. This study suggests DHM as a novel marker-free nonperturbing method to study lipid droplet accumulation and may be envisioned for drug screens and mechanistic studies on adipocytic differentiation.

Published

2018

30. Image-Based Marker-Free Screening of GABA

Author

Benjamin, Rappaz, Pascal, Jourdain, Damiano, Banfi, Fabien, Kuttler, Pierre, Marquet, and Gerardo, Turcatti

Subjects

Biological Products, Microscopy, quantitative phase imaging, Holography, ligand-gated ion channels, digital holographic microscopy, GABAA, Receptors, GABA-A, high-content screening, Article, Electrophysiological Phenomena, High-Throughput Screening Assays, Molecular Imaging, Image Processing, Computer-Assisted, Humans, GABA-A Receptor Agonists, GABA-A Receptor Antagonists, gamma-Aminobutyric Acid

Abstract

The ionotropic GABAA receptors represent the main target for different groups of widely used drugs having hypnotic and anxiolytic effects. So far, most approaches used to assess GABA activity involve invasive low -throughput electrophysiological techniques or rely on fluorescent dyes, preventing the ability to conduct noninvasive and thus nonperturbing screens. To address this limitation, we have developed an automated marker-free cell imaging method, based on digital holographic microscopy (DHM). This technology allows the automatically screening of compounds in multiple plates without having to label the cells or use special plates. This methodological approach was first validated by screening the GABAA receptor expressed in HEK cells using a selection of active compounds in agonist, antagonist, and modulator modes. Then, in a second blind screen of a library of 3041 compounds (mostly composed of natural products), 5 compounds having a specific agonist action on the GABAA receptor were identified. The hits validated from this unbiased screen were the natural products muscimol, neurosteroid alphaxalone, and three compounds belonging to the avermectin family, all known for having an agonistic effect on the GABAA receptor. The results obtained were exempt from false negatives (structurally similar unassigned hits), and false-positive hits were detected and discarded without the need for performing electrophysiological measurements. The outcome of the screen demonstrates the applicability of our screening by imaging method for the discovery of new chemical structures, particularly regarding chemicals interacting with the ionotropic GABAA receptor and more generally with any ligand-gated ion channels and transporters.

Published

2019

31. Loss of Bacterial Cell Pole Stabilization in Caulobacter crescentus Sensitizes to Outer Membrane Stress and Peptidoglycan-Directed Antibiotics

Author

Clare L. Kirkpatrick, Simon Ulysse Vallet, Freja Cecillie Bistrup, Patrick H. Viollier, Gerardo Turcatti, Lykke Haastrup Hansen, Julien Bortoli Chapalay, and Marc Chambon

Subjects

Cell wall, chemistry.chemical_compound, biology, Chemistry, Caulobacter crescentus, Peptidoglycan, Polar organelle, Cell envelope, biology.organism_classification, Bacterial outer membrane, Intracellular, Bacterial cell structure, Cell biology

Abstract

Rod-shaped bacteria frequently localise proteins to one or both cell poles in order to regulate processes such as chromosome replication or polar organelle development. However, the role of such polar factors in responses to extracellular stimuli has been generally unexplored. We employed chemical-genetic screening to probe the interaction between one such factor fromCaulobacter crescentus, TipN, and extracellular stress and found that TipN is required for normal tolerance of cell envelope-directed antibiotics, including vancomycin that does not normally inhibit growth of Gram-negative bacteria. Forward genetic screening for suppressors of vancomycin sensitivity in the absence of TipN revealed the TonB-dependent receptor ChvT as the mediator of vancomycin tolerance. Loss of ChvT improved resistance to vancomycin and cefixime in the otherwise sensitive ΔtipNstrain. The activity of the two-component system regulating ChvT (ChvIG) was increased in ΔtipNcells relative to wild type under some, but not all, cell wall stress conditions that this strain was sensitised to, in particular cefixime and detergent exposure. Together, these results indicate that the ChvIG two-component system has been co-opted as a sensor of cell wall stress and that TipN can influence cell envelope stability and ChvIG-mediated signaling in addition to its roles in intracellular development.Author summaryMaintenance of an intact cell envelope is essential for free-living bacteria to survive harsh conditions they may encounter in their environment. In the case of rod-shaped bacteria, the poles of the cell are potential weak points in the cell envelope due to the high curvature of the layers and the need to break and re-form parts of the cell envelope at the division plane in order to form new poles as the cells replicate and divide. We have found that TipN, a factor required for correct division and cell pole development in the rod-shaped bacterium,Caulobacter crescentus, is also needed for maintaining normal levels of resistance to cell wall-targeting antibiotics such as vancomycin and cefixime, which interfere with peptidoglycan synthesis. We also identified an outer membrane receptor, ChvT, that was responsible for allowing vancomycin access to the cells and found that the two-component system that negatively regulates ChvT production was activated by various kinds of cell wall stress. Presence or absence of TipN influenced how active this system was in the presence of cefixime or of the membrane-disrupting detergent sodium deoxycholate. Since TipN is normally located at the poles of the cell and at the division plane just before cells complete division, our results suggest that it is involved in stabilisation of these weak points of the cell envelope as well as its other roles inside the cell.

Published

2019

32. Wnt directs the endosomal flux of <scp>LDL</scp> ‐derived cholesterol and lipid droplet homeostasis

Author

Jean Gruenberg, Fabrizio Vacca, Stefania Vossio, Cameron C. Scott, Olivier Schaad, Jorge Larios, Marc Chambon, Lucas Pelkmans, Dmitry Kuznetsov, Olivier Martin, Gerardo Turcatti, Nicolas Guex, Berend Snijder, University of Zurich, and Gruenberg, Jean

Subjects

1303 Biochemistry, Endosome, lipid droplets, Biology, Endocytosis, Biochemistry, Cell Line, Mice, chemistry.chemical_compound, L Cells, 1311 Genetics, Wnt3A Protein, Lipid droplet, 1312 Molecular Biology, Genetics, Animals, Homeostasis, Humans, LDL-derived cholesterol, Wnt Signaling Pathway, Molecular Biology, Cholesterol, Gene Expression Profiling, Wnt signaling pathway, Epithelial Cells, Cholesterol, LDL, Articles, 10124 Institute of Molecular Life Sciences, High-Throughput Screening Assays, Cell biology, chemistry, endosomes, canonical Wnt signaling, Nanophotonics, Plasmonics, 570 Life sciences, biology, RNA Interference, lipids (amino acids, peptides, and proteins), functional genomics, Flux (metabolism), WNT3A, HeLa Cells, Oleic Acid

Abstract

The Wnt pathway, which controls crucial steps of the development and differentiation programs, has been proposed to influence lipid storage and homeostasis. In this paper, using an unbiased strategy based on high-content genome-wide RNAi screens that monitored lipid distribution and amounts, we find that Wnt3a regulates cellular cholesterol. We show that Wnt3a stimulates the production of lipid droplets and that this stimulation strictly depends on endocytosed, LDL-derived cholesterol and on functional early and late endosomes. We also show that Wnt signaling itself controls cholesterol endocytosis and flux along the endosomal pathway, which in turn modulates cellular lipid homeostasis. These results underscore the importance of endosome functions for LD formation and reveal a previously unknown regulatory mechanism of the cellular programs controlling lipid storage and endosome transport under the control of Wnt signaling.

Published

2015

33. Development of a semi-automated image-based high-throughput drug screening system

Author

Julien Bortoli Chapalay, Marc Chambon, Dimitri Moreau, Nicolas Fasel, Lon-Fye Lye, Dmitry Kopelyanskiy, Remzi Onur Eren, Stephen M. Beverley, and Gerardo Turcatti

Subjects

0301 basic medicine, Drug, media_common.quotation_subject, 030106 microbiology, Antiprotozoal Agents, Drug Evaluation, Preclinical, Biology, General Biochemistry, Genetics and Molecular Biology, Article, Chemical library, Pathogenesis, 03 medical and health sciences, chemistry.chemical_compound, Automation, Mice, High-Throughput Screening Assays, Animals, Antiprotozoal Agents/pharmacology, Drug Evaluation, Preclinical/methods, Leishmania/drug effects, Macrophages/parasitology, Mice, Inbred C57BL, Parasite hosting, media_common, Leishmania, General Immunology and Microbiology, Macrophages, RNA virus, biology.organism_classification, Virology, Drug repositioning, chemistry

Abstract

We previously reported that the innate sensing of the endosymbiont Leishmania RNA virus 1 (LRV1) within Leishmania (Viannia) guyanensis through Toll-like receptor 3, worsens the pathogenesis of parasite infection in mice. The presence of LRV1 has been associated with the failure of first-line treatment in patients infected with LRV1 containing - L. guyanensis and - L. braziliensis parasites. Here, we established a semi-automated image-based high-throughput drug screening (HTDS) protocol to measure parasiticidal activity of the Prestwick chemical library in primary murine macrophages infected with LRV1-containing L. guyanensis . The two-independent screens generated 14 hit compounds with over sixty-nine percent reduction in parasite growth compared to control, at a single dose in both screens. Our screening strategy offers great potential in the search for new drugs and accelerates the discovery rate in the field of drug repurposing against Leishmania . Moreover, this technique allows the concomitant assessment of the effect of drug toxicity on host cell number.

Published

2018

34. A new class of cleavable fluorescent nucleotides: synthesis and optimization as reversible terminators for DNA sequencing by synthesis

Author

Milan Fedurco, Gerardo Turcatti, Ana-Paula Tairi, and Anthony Romieu

Subjects

Sequence analysis, Deoxyribonucleotides, Biology, DNA sequencing, Fluorescence, chemistry.chemical_compound, Genetics, Organic Chemicals/chemistry, Nucleotide, Organic Chemicals, Protecting group, Alexa Fluor, Fluorescent Dyes, chemistry.chemical_classification, Microscopy, Deoxyribonucleotides/classification, Deoxyribonucleotides/chemistry, Sequence Analysis, DNA, Fluorescent Dyes/chemistry, Deoxyribonucleotides/chemical synthesis, DNA, genomic DNA, chemistry, Biochemistry, Microscopy, Fluorescence, Methods Online, Sequence Analysis

Abstract

Fluorescent 2'-deoxynucleotides containing a protecting group at the 3'-O-position are reversible terminators enabling array-based DNA sequencing by synthesis (SBS) approaches. Herein, we describe the synthesis of a new family of 3'-OH unprotected cleavable fluorescent 2'-deoxynucleotides and their evaluation as reversible terminators for high-throughput DNA SBS strategies. In this first version, all four modified nucleotides bearing a cleavable disulfide Alexa Fluor(R) 594 dye were assayed for their ability to act as a reversible stop for the incorporation of the next labeled base. Their use in SBS leaded to a signal-no signal output after successive addition of each labeled nucleotide during the sequencing process (binary read-out). Solid-phase immobilized synthetic DNA target sequences were used to optimize the method that has been applied to DNA polymerized colonies or clusters obtained by in situ solid-phase amplification of fragments of genomic DNA templates.

Published

2017

35. Digital Holographic Microscopy: A Quantitative Label-Free Microscopy Technique for Phenotypic Screening

Author

Gerardo Turcatti, Billy Breton, Etienne Shaffer, and Benjamin Rappaz

Subjects

Microscope, Holography, differential interference contrast, Nanotechnology, Image processing, Biology, high-content screening, Cell morphology, Time-Lapse Imaging, digital holography, phase contrast, Article, Cell Line, law.invention, law, Drug Discovery, Microscopy, Image Processing, Computer-Assisted, Animals, Humans, Microscopy, Phase-Contrast, Myocytes, Cardiac, Cytotoxins, Organic Chemistry, Chloroquine, General Medicine, Rats, Computer Science Applications, phenotypic drug discovery, Phenotype, Differential interference contrast microscopy, Doxorubicin, High-content screening, ion channel, image-based screen, Cell-based assay, Biological Assay, Digital holographic microscopy, Digital holography, HeLa Cells, Biomedical engineering

Abstract

Digital Holographic Microscopy (DHM) is a label-free imaging technique allowing visualization of transparent cells with classical imaging cell culture plates. The quantitative DHM phase contrast image provided is related both to the intracellular refractive index and to cell thickness. DHM is able to distinguish cellular morphological changes on two representative cell lines (HeLa and H9c2) when treated with doxorubicin and chloroquine, two cytotoxic compounds yielding distinct phenotypes. We analyzed parameters linked to cell morphology and to the intracellular content in endpoint measurements and further investigated them with timelapse recording. The results obtained by DHM were compared with other optical label-free microscopy techniques, namely Phase Contrast, Differential Interference Contrast and Transport of Intensity Equation (reconstructed from three bright-field images). For comparative purposes, images were acquired in a common 96-well plate format on the different motorized microscopes. In contrast to the other microscopies assayed, images generated with DHM can be easily quantified using a simple automatized on-the-fly analysis method for discriminating the different phenotypes generated in each cell line. The DHM technology is suitable for the development of robust and unbiased image-based assays.

Published

2014

36. Label-Free Cytotoxicity Screening Assay by Digital Holographic Microscopy

Author

Christian Depeursinge, Julien Mena, Marc Chambon, Pierre Marquet, Billy Breton, Jonas Kühn, Etienne Shaffer, Jérôme Parent, Yves Emery, Pierre J. Magistretti, Gerardo Turcatti, and Benjamin Rappaz

Subjects

Materials science, Microscope, Phenotypic screening, Drug Evaluation, Preclinical, Holography, Nanotechnology, Sensitivity and Specificity, 01 natural sciences, law.invention, 010309 optics, 03 medical and health sciences, Imaging, Three-Dimensional, law, Image Interpretation, Computer-Assisted, Toxicity Tests, 0103 physical sciences, Drug Discovery, Microscopy, Fluorescence microscope, Viability assay, Cytotoxicity, 030304 developmental biology, 0303 health sciences, Staining and Labeling, Reproducibility of Results, Signal Processing, Computer-Assisted, Equipment Design, Original Articles, Equipment Failure Analysis, Microscopy, Fluorescence, High-content screening, Molecular Medicine, Biological Assay, Digital holographic microscopy, Biomedical engineering

Abstract

We introduce a label-free technology based on digital holographic microscopy (DHM) with applicability for screening by imaging, and we demonstrate its capability for cytotoxicity assessment using mammalian living cells. For this first high content screening compatible application, we automatized a digital holographic microscope for image acquisition of cells using commercially available 96-well plates. Data generated through both label-free DHM imaging and fluorescence-based methods were in good agreement for cell viability identification and a Z′-factor close to 0.9 was determined, validating the robustness of DHM assay for phenotypic screening. Further, an excellent correlation was obtained between experimental cytotoxicity dose–response curves and known IC50 values for different toxic compounds. For comparable results, DHM has the major advantages of being label free and close to an order of magnitude faster than automated standard fluorescence microscopy.

Published

2013

37. Red blood cells ageing markers: a multi-parametric analysis

Author

Manon, Bardyn, Benjamin, Rappaz, Keyvan, Jaferzadeh, David, Crettaz, Jean-Daniel, Tissot, Inkyu, Moon, Gerardo, Turcatti, Niels, Lion, and Michel, Prudent

Subjects

Oxidative Stress, Erythrocytes, Glucose, Blood Preservation, Cell-Derived Microparticles, Humans, Original Article, Citrates, Erythrocyte Aging, Lactic Acid, Glutathione, Hemolysis, Oxidation-Reduction

Abstract

Red blood cells collected in citrate-phosphate-dextrose can be stored for up to 42 days at 4 °C in saline-adenine-glucose-mannitol additive solution. During this controlled, but nevertheless artificial, ex vivo ageing, red blood cells accumulate lesions that can be reversible or irreversible upon transfusion. The aim of the present study is to follow several parameters reflecting cell metabolism, antioxidant defences, morphology and membrane dynamics during storage.Five erythrocyte concentrates were followed weekly during 71 days. Extracellular glucose and lactate concentrations, total antioxidant power, as well as reduced and oxidised intracellular glutathione levels were quantified. Microvesiculation, percentage of haemolysis and haematologic parameters were also evaluated. Finally, morphological changes and membrane fluctuations were recorded using label-free digital holographic microscopy.The antioxidant power as well as the intracellular glutathione concentration first increased, reaching maximal values after one and two weeks, respectively. Irreversible morphological lesions appeared during week 5, where discocytes began to transform into transient echinocytes and finally spherocytes. At the same time, the microvesiculation and haemolysis started to rise exponentially. After six weeks (expiration date), intracellular glutathione was reduced by 25%, reflecting increasing oxidative stress. The membrane fluctuations showed decreased amplitudes during shape transition from discocytes to spherocytes.Various types of lesions accumulated at different chemical and cellular levels during storage, which could impact their in vivo recovery after transfusion. A marked effect was observed after four weeks of storage, which corroborates recent clinical data. The prolonged follow-up period allowed the capture of deep storage lesions. Interestingly, and as previously described, the severity of the changes differed among donors.

Published

2016

38. Screening out irrelevant cell-based models of disease

Author

Spencer L. Shorte, Nathalie Aulner, Carina von Schantz, Peter Horvath, Gerardo Turcatti, Marc Bickle, María C. Montoya, Päivi Östling, Neil O. Carragher, Daniel Ebner, Vilja Pietiäinen, Elaine Del Nery, Anthony Davies, and Leo S. Price

Subjects

0301 basic medicine, Induced Pluripotent Stem Cells, Cell Culture Techniques, Drug Evaluation, Preclinical, Translational research, Drug development, Disease, Bioinformatics, Models, Biological, 03 medical and health sciences, Genome editing, Multidisciplinary approach, High-Throughput Screening Assays, Drug Discovery, Medicine, Animals, Humans, Induced pluripotent stem cell, Cell Line, Transformed, Pharmacology, Drug discovery, business.industry, Small molecules, General Medicine, Data science, 3. Good health, 030104 developmental biology, Pharmaceutical Preparations, Drug screening, business

Abstract

The common and persistent failures to translate promising preclinical drug candidates into clinical success highlight the limited effectiveness of disease models currently used in drug discovery. An apparent reluctance to explore and adopt alternative cell- and tissue-based model systems, coupled with a detachment from clinical practice during assay validation, contributes to ineffective translational research. To help address these issues and stimulate debate, here we propose a set of principles to facilitate the definition and development of disease-relevant assays, and we discuss new opportunities for exploiting the latest advances in cell-based assay technologies in drug discovery, including induced pluripotent stem cells, three-dimensional (3D) co-culture and organ-on-a-chip systems, complemented by advances in single-cell imaging and gene editing technologies. Funding to support precompetitive, multidisciplinary collaborations to develop novel preclinical models and cell-based screening technologies could have a key role in improving their clinical relevance, and ultimately increase clinical success rates.

Published

2016

39. Quantification of stored red blood cell fluctuations by time-lapse holographic cell imaging

Author

Jean-Daniel Tissot, Michel Prudent, Pierre Marquet, Benjamin Rappaz, Bahram Javidi, Inkyu Moon, Manon Bardyn, Keyvan Jaferzadeh, and Gerardo Turcatti

Subjects

0301 basic medicine, Whole membrane, human erythrocytes, refractive-index, Materials science, Mean corpuscular hemoglobin, membrane fluctuations, digital holography, 01 natural sciences, Article, Sphericity, storage, 010309 optics, 03 medical and health sciences, Dimple, 0103 physical sciences, Microscopy, medicine, Mean corpuscular volume, Millisecond, medicine.diagnostic_test, dynamics, contrast, Atomic and Molecular Physics, and Optics, Red blood cell, 030104 developmental biology, medicine.anatomical_structure, microscopy, identification, living cells, Biotechnology, Biomedical engineering

Abstract

We propose methods to quantitatively calculate the fluctuation rate of red blood cells with nanometric axial and millisecond temporal sensitivity at the single-cell level by using time-lapse holographic cell imaging. For this quantitative analysis, cell membrane fluctuations (CMFs) were measured for RBCs stored at different storage times. Measurements were taken over the whole membrane for both the ring and dimple sections separately. The measurements show that healthy RBCs that maintain their discocyte shape become stiffer with storage time. The correlation analysis demonstrates a significant negative correlation between CMFs and the sphericity coefficient, which characterizes the morphological type of erythrocyte. In addition, we show the correlation results between CMFs and other morphological properties such as projected surface area, surface area, mean corpuscular volume, and mean corpuscular hemoglobin. (C) 2018 Optical Society of America under the terms of the OSA Open Access Publishing Agreement

Published

2018

40. Cell-based high-content screening with label-free Digital Holographic Imaging

Author

Fabien Kuttler, Gerardo Turcatti, and Benjamin Rappaz

Abstract

We automated a system for performing quantitative cellular assays using label-free Digital Holographic Microscopy (DHM) and validated its applicability for cell viability assays in a drug screening context 1-2. Our system allows performing fast and cost-effective screening assays for a wide range of chemical biology and drug discovery applications. In addition to classic phenotypes recordings related to morphological changes and cell movements, we have demonstrated that target-based cellular assays can also be addressed by DHM for therapeutically relevant chloride channel receptors 3. DH-imaging (DHI) technology, scalable for screening by imaging approaches in a high-throughput manner can also deliver highly informative data through long term experiments (time lapse). Examples of label free imaging screens we validated or currently under development will be described:Profiling cancer cell-line sensitivities with small moleculesMonitoring the activity of the GABA A chloride channel receptor ('an optical electrode')Assessing cardiotoxycity of compounds using human cardiomyocytes derived from induced pluripotent stem cells (iPSCs) 4.

Published

2015

41. Automated multi-parameter measurement of cardiomyocytes dynamics withdigital holographic microscopy

Author

Benjamin Rappaz, Pierre Marquet, Inkyu Moon, Bahram Javidi, Faliu Yi, and Gerardo Turcatti

Subjects

Signal processing, business.industry, Computer science, Atomic force microscopy, Dynamics (mechanics), Nanotechnology, Atomic and Molecular Physics, and Optics, Interference microscopy, Optics, Optical imaging, Drug development, Feature (computer vision), Three-dimensional image processing Cell analysis Medical and biological imaging Digital holography, Digital holographic microscopy, business, Biological system, Multi parameter

Abstract

Compounds tested during drug development may have adverse effects on the heart; therefore all new chemical entities have to undergo extensive preclinical assessment for cardiac liability. Conventional intensity-based imaging techniques are not robust enough to provide detailed information for cell structure and the captured images result in lowcontrast, especially to cell with semi-transparent or transparent feature, which would affect the cell analysis. In this paper we show, for the first time, that digital holographic microscopy (DHM) integrated with information processing algorithms automatically provide dynamic quantitative phase profiles of beating cardiomyocytes. We experimentally demonstrate that relevant parameters of cardiomyocytes can be obtained by our automated algorithm based on DHM phase signal analysis and used to characterize the physiological state of resting cardiomyocytes. Our study opens the possibility of automated quantitative analysis of cardiomyocyte dynamics suitable for further drug safety testing and compounds selection as a new paradigm in drug toxicity screens. (C) 2015 Optical Society of America

Published

2015

42. Digital Holographic Imaging for Label-Free Phenotypic Profiling, Cytotoxicity, and Chloride Channels Target Screening

Author

Gerardo Turcatti, Fabien Kuttler, Benjamin Rappaz, Billy Breton, and Fang, Ye

Subjects

medicine.anatomical_structure, Cell growth, Cell, Cell migration - Cell proliferation - CFTR - Chloride channels - Cytotoxicity profiling - Digital holographic microscopy - GABAA - High-content screening - Label-free quantitative microscopy - Phenotypic drug discovery, Chloride channel, medicine, Digital holographic microscopy, Viability assay, Biology, Cytotoxicity, Receptor, Phenotype, Cell biology

Abstract

Cellular assays using label-free Digital Holographic Microscopy (DHM) have been previously validated for cell viability assays in a drug screening context. Our automated DHM system allows performing fast and cost-effective screening assays for a wide range of applications for monitoring cell morphological changes and cell movements upon interaction with interfering compounds. In addition to these classic phenotypic assays, it has been demonstrated that target-based cellular assays can also be addressed by DHM for therapeutically relevant chloride channel receptors. Our DH-imaging (DHI) technology, potentially scalable for screening by imaging approaches in a high-throughput manner can also deliver highly informative data through long term experiments. Three examples of phenotypic screens are detailed in the present chapter: a label-free profiling approach, a cell proliferation assay, and methods for monitoring the activity of the GABAA chloride channel receptor.

Published

2015

43. [Untitled]

Author

Gerardo Turcatti and André Chollet

Subjects

biology, Chemistry, G protein, Structure function, Computational biology, Guanine Nucleotide Binding Protein, Computer Science Applications, Order (biology), Biochemistry, Rhodopsin, Drug Discovery, biology.protein, Physical and Theoretical Chemistry, Receptor, Receptor activation, G protein-coupled receptor

Abstract

G protein-coupled receptors (GPCR) represent a large family of drug targets for which there is no high-resolution structural information. In order to understand the mechanisms of ligand recognition and receptor activation, there is a strong need for novel biophysical methods. In this perspective we provide an overview of recent experimental approaches used to explore the molecular architecture and dynamics of GPCR and their interactions with ligands and G proteins using biophysical, non-crystallographic, methods.

Published

1999

44. Developing the Biomolecular Screening Facility at the EPFL into the Chemical Biology Screening Platform for Switzerland

Author

Gerardo Turcatti

Subjects

Engineering, assay development, Biomedical Research, Systems biology, target-based assays, Chemical biology, Nanotechnology, hits-to-leads, high-content screening, Drug Discovery, Applied research, RNA, Small Interfering, Competence (human resources), assay automation, Drug discovery, business.industry, Organic Chemistry, Academic screening, General Medicine, Computer Science Applications, Chemical screening, High-Throughput Screening Assays, Engineering management, High-content screening, phenoytpic assays, Workforce, hits prioritization, business, Chemical genetics, Switzerland

Abstract

The Biomolecular Screening Facility (BSF) is a multidisciplinary laboratory created in 2006 at the Ecole Polytechnique Federale de Lausanne (EPFL) to perform medium and high throughput screening in life sciences-related projects. The BSF was conceived and developed to meet the needs of a wide range of researchers, without privileging a particular biological discipline or therapeutic area. The facility has the necessary infrastructure, multidisciplinary expertise and flexibility to perform large screening programs using small interfering RNAs (siRNAs) and chemical collections in the areas of chemical biology, systems biology and drug discovery. In the framework of the National Centres of Competence in Research (NCCR) Chemical Biology, the BSF is hosting 'ACCESS', the Academic Chemical Screening Platform of Switzerland that provides the scientific community with chemical diversity, screening facilities and know-how in chemical genetics. In addition, the BSF started its own applied research axes that are driven by innovation in thematic areas related to preclinical drug discovery and discovery of bioactive probes.

Published

2013

45. Telomerase inhibitors from cyanobacteria: isolation and synthesis of sulfoquinovosyl diacylglycerols from Microcystis aeruguinosa PCC 7806

Author

Karl Gademann, Tom M. Woods, Joachim Lingner, Danilo D’Ambrosio, Cyril Portmann, Patrick Reichenbach, Damiano Banfi, Gerardo Turcatti, Emilie Baudat, Laeticia Da Silva, and Malika Makhlouf Brahmi

Subjects

Cyanobacteria, Telomerase, Microcystis, Phencyclidine, Tandem mass spectrometry, 01 natural sciences, Catalysis, Diglycerides, 03 medical and health sciences, Structure-Activity Relationship, Tandem Mass Spectrometry, Structure–activity relationship, Enzyme Inhibitors, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, Chromatography, biology, 010405 organic chemistry, Organic Chemistry, Biological activity, General Chemistry, biology.organism_classification, 0104 chemical sciences, Enzyme, Biochemistry, chemistry, Glycolipids, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

By using the Telospot assay, 27 different extracts of cyanobacteria were evaluated for telomerase inhibition. All extracts showed varying, but significant activity. We selected Microcystis aeruguinosa PCC 7806 to identify the active compound and a bioassay guided fractionation led us to isolate mixtures of sulfoquinovosyl diacylglycerols (SQDGs), which were identified by 2D NMR and MS/MS experiments. Pure SQDG derivatives were then synthesized. The IC(50) values of pure synthetic sulfoquinovosyl dipalmitoylglycerol and the monopalmitoylated derivative against telomerase were determined to be 17 and 40 μM, respectively. A structure-activity relationship study allowed the identification of compounds with modified lipophilic acyl groups that display improved activity.

Published

2013

46. Abstract 338: A novel small molecule inhibitor of the Notch transcription activation complex

Author

Rajwinder Lehal, Freddy Radtke, Gerardo Turcatti, Sylvain Loubéry, Jean-Pierre Bourquin, Viktoria Reinmuller, Marcos González-Gaitán, and Viktoras Frismantas

Subjects

Fusion gene, Cancer Research, Programmed cell death, Oncology, Chemistry, Muscle cell differentiation, Notch signaling pathway, Receptor, Small molecule, Phenotype, Triple-negative breast cancer, Cell biology

Abstract

NOTCH signaling is a developmental pathway known to play critical roles during embryonic development as well as for the regulation of self-renewing tissues. Aberrant activation of NOTCH signaling leads to deregulation of the self-renewal process resulting in sustained proliferation, evasion of cell death, loss of differentiation capacity, invasion and metastasis, all of which are hallmarks of cancer. Over activation of NOTCH in human cancers can be a consequence of over expression of NOTCH ligands/receptors, GOF mutations in NOTCH receptors as well as chromosomal translocations leading to constitutive activation of the pathway. Given the importance of Notch signaling in human cancers, several therapeutic approaches have been utilized to block NOTCH signaling. Two of these strategies are; a) the use of monoclonal blocking antibodies (Mabs) against NOTCH ligands and receptors and b) the use of small molecule γ-secretase inhibitors (GSIs). However, these approaches can only be effective if tumor cells express full-length ligand or receptor molecules. On the contrary, in human cancers harbouring NOTCH gene fusion due to chromosomal translocations, the use of Mabs and GSIs will have very limited clinical benefits. A third, yet not fully explored approach could be the blockage of NOTCH signalling by targeting the most downstream event in the NOTCH cascade i,e NOTCH transcriptional activation complex using small molecule inhibitors. Here we report discovery and identification of a novel, orally-active small molecule inhibitor, named CB-103, of the NOTCH pathway that blocks NOTCH signaling by targeting the NOTCH transcriptional activation complex in the nucleus. CB-103 has shown the ability to block NOTCH signalling in human cancer cell lines, induce neurogenic phenotype in drosophila, induce muscle cell differentiation and inhibit NOTCH dependent cellular processes in mice. In addition, CB-103 exhibit anti-tumor efficacy in a xenograft model of human triple negative breast cancer resistant to GSIs and Mabs against NOTCH ligands/receptors. Furthermore, CB-103 has shown a remarkable activity in PDX models of human T-ALL harbouring activation of the NOTCH pathway. Additional studies are underway on several analogs of CB-103 to determine ADME/PK/PD profile and nominate a development candidate for further clinical development of this novel inhibitor of the NOTCH pathway. Citation Format: Rajwinder Lehal, Viktoras Frismantas, Sylvain Loubéry, Viktoria Reinmuller, Gerardo Turcatti, Marcos Gonzalez-Gaitan, Jean-Pierre Bourquin, Freddy Radtke. A novel small molecule inhibitor of the Notch transcription activation complex. [abstract]. In: Proceedings of the 107th Annual Meeting of the American Association for Cancer Research; 2016 Apr 16-20; New Orleans, LA. Philadelphia (PA): AACR; Cancer Res 2016;76(14 Suppl):Abstract nr 338.

Published

2016

47. Chemical biology approaches to membrane homeostasis and function

Author

Robbie Loewith, Gerardo Turcatti, Andreas Zumbuehl, Howard Riezman, Stefan Matile, Kai Johnsson, Ludovic Pineau, David Alonso Doval, Aurélien Roux, Christian Heinis, Miwa Takahashi-Umebayashi, Thomas Hannich, and Luc Reymond

Subjects

SPHINGOLIPIDS, MEMBRANES, 01 natural sciences, Fluorescent dyes, Cell membrane, Rafts, Homeostasis, Turning point, RAFTS, STEROLS, 0303 health sciences, Neuropathy Type-I, General Medicine, CHEMICAL BIOLOGY, Chemical biology, Cell biology, Chemistry, Sterols, medicine.anatomical_structure, Membrane, SIGNALING, ddc:540, Domains, Giant unilamellar vesicles, Mutations, Subunit, GIANT UNILAMELLAR VESICLES, Microdomains, Membrane lipids, Computational biology, Biology, Gpi-Anchored Proteins, Article, 03 medical and health sciences, Membrane Lipids, INSULIN RECEPTOR, ddc:570, medicine, QD1-999, 030304 developmental biology, MICRODOMAINS, FLUORESCENT DYES, Sphingolipids, Membranes, 010405 organic chemistry, Cell Membrane, Membrane structure, General Chemistry, Signaling, 0104 chemical sciences, Function (biology), Insulin receptor

Abstract

The study of membranes is at a turning point. New theories about membrane structure and function have recently been proposed, however, new technologies, combining chemical, physical, and biochemical approaches are necessary to test these hypotheses. In particular, the NCCR in chemical biology aims to visualize and characterize membrane microdomains and determine their function during hormone signaling.

Published

2012

48. Purification cDNA cloning and heterologous expression of human phosphomannose isomerase

Author

David Smith, Gerardo Turcatti, Timothy N. C. Wells, Mark A. Payton, and Amanda E. I. Proudfoot

Subjects

DNA, Complementary, Placenta, Genes, Fungal, Molecular Sequence Data, Restriction Mapping, Gene Expression, Saccharomyces cerevisiae, Isomerase, Biology, Molecular cloning, Biochemistry, Pregnancy, Complementary DNA, Escherichia coli, Humans, Amino Acid Sequence, Cloning, Molecular, Promoter Regions, Genetic, Peptide sequence, Mannose-6-Phosphate Isomerase, Base Sequence, Sequence Homology, Amino Acid, Muscles, Myocardium, Mannose phosphate isomerase, Nucleic acid sequence, Brain, Molecular biology, Peptide Fragments, Recombinant Proteins, Kinetics, Organ Specificity, Chromatography, Gel, Female, Heterologous expression, Plasmids

Abstract

Phosphomannose isomerase catalyses the interconversion of fructose-6-P and mannose-6-P and has a critical role in the supply of D-mannose derivatives required for many eukaryotic glycosylation reactions. Three classes of enzymes possessing phosphomannose-isomerase activity have been identified in bacteria and lower eukaryotes. We have purified human phosphomannose isomerase to homogeneity from placental tissue. Protein sequence information obtained from internal fragments of the protein was used to design degenerate oligonucleotides which were used to amplify a fragment of a human phosphomannose-isomerase cDNA. A full-length cDNA was isolated from a human testes lambda gt11 library using this fragment as a probe. The cDNA encoded a protein with significant sequence identity to fungal and some bacterial phosphomannose isomerases but was unrelated to those from other bacteria. Based on amino acid sequence identity we propose a classification system for enzymes with phosphomannose-isomerase activity. The cDNA, under the control of the GAL1 promoter, was expressed in a Saccharomyces cerevisiae strain from which the native gene encoding phosphomannose isomerase had been deleted. The human enzyme was found to be able to functionally substitute for the yeast enzyme. Phosphomannose-isomerase mRNA was found in all human tissues tested but was more highly expressed in heart, brain and skeletal muscle. The cDNA was expressed in Escherichia coli permitting the isolation of pure recombinant protein which will be used for kinetic and structural studies.

Published

1994

49. Role of cysteine62in DNA recognition by the P50 subunit of NF-xB

Author

Wiweka Kaszubska, James R. Matthews, Ronald T. Hay, Gerardo Turcatti, and Timothy N. C. Wells

Subjects

DNA, Bacterial, HMG-box, Protein subunit, Molecular Sequence Data, Mutant, Biology, chemistry.chemical_compound, Escherichia coli, Genetics, Amino Acid Sequence, Cysteine, Cloning, Molecular, Binding site, Binding Sites, DNA clamp, Base Sequence, Oligonucleotide, NF-kappa B, Molecular biology, DNA binding site, Kinetics, chemistry, Biochemistry, Mutation, Oxidation-Reduction, DNA

Abstract

A powerful chemical modification procedure has been developed to define determinants of DNA recognition by the p50 subunit of NF-kappa B. Differential labelling with [14C] iodoacetate has identified a conserved cysteine residue, Cys62, that was protected from modification by the presence of an oligonucleotide containing the specific recognition site of the protein. To determine the importance of this cysteine residue, each of the conserved cysteines in p50 was changed to serine and the DNA binding properties of the mutant proteins determined. Scatchard analysis indicated that the C62S mutant bound to its DNA recognition site with a 10-fold larger dissociation constant than the wild type protein, while the other two mutants bound with an intermediate affinity. Dissociation rate constant measurements correlated well with the dissociation constants for the wild type, C119S, and C273S p50 proteins, whereas the p50 C62S-DNA complex dissociated anomalously quickly. Competition analyses with oligonucleotide variants of the DNA recognition site and nonspecific E. coli DNA revealed that the C62S p50 mutant had an altered DNA binding site specificity and was impaired in its ability to discriminate between specific and non-specific DNA. Thus the sulphydryl group of Cys62 is an important determinant of DNA recognition by the p50 subunit of NF-kappa B.

Published

1993

50. Partial characterization of natural and recombinant human soluble CD23

Author

Gerardo Turcatti, N Aubonney, Pierre Graber, P O Regamey, S Pochon, J Y Bonnefoy, Keith Rose, E Magnenat, and K U Jansen

Subjects

Stereochemistry, Molecular Sequence Data, Peptide Mapping, Biochemistry, Mass Spectrometry, law.invention, Residue (chemistry), Protein structure, law, protein purification, Protein purification, Humans, Trypsin, Amino Acid Sequence, Disulfides, protein structure, Molecular Biology, Peptide sequence, Polyacrylamide gel electrophoresis, Protein secondary structure, Chromatography, High Pressure Liquid, Edman degradation, Receptors, IgE, Chemistry, Cell Biology, Immunoglobulin E, Recombinant Proteins, protein analysis, Recombinant DNA, cd23 antigen, Electrophoresis, Polyacrylamide Gel, Research Article

Abstract

The purification to homogeneity of an active soluble 25 kDa fragment of CD23, produced in insect cells using the baculovirus expression system, is described. Peptide mapping and analysis by Edman degradation and mass spectrometry permitted partial characterization of the protein. A total of 165 out of 172 residues, including N-terminal and C-terminal regions, were mapped. The positions of the two disulphide bonds in the IgE-binding region were also determined: residue 110 is joined to residue 124, and residue 42 to residue 133. Natural CD23 25 kDa fragment was also analysed and found to possess the same disulphide bond arrangement. These results extend the previously noted sequence similarity with lectins to elements of secondary structure.

Published

1992