High Content Imaging : Meaningful pictures for relevant results in dermocosmetology

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High Content Imaging : Meaningful pictures for relevant results in dermocosmetology We deliver High Content screening services with exhaustive, high quality and robust phenotypic data. Nathalie MAUBON, CEO at HCS Pharma

Custom Assay Development On Demand 1 CHOOSE YOUR CELL CULTURE SYSTEM 2D 3D 96 or 384-well plates ULA plates BIOMIMESYS Cell lines Adipocyte in BIOMIMESYS Primary cells or IPS e.g. keratinocytes e.g. hepatocytes Keratinocytes Fibroblastes Melanocytes Macrophages Reconstructed skin 2 - CHOOSE YOUR INDUCERS & INCUBATION TIME Fixed Cells Live Cells Small Molecules Biologicals Ingredients Starvations UV Radiations

Custom Assay Development On Demand 3 CHOOSE YOUR READ-OUTS Proliferation, apoptosis, Cell motility (tracking) Extra-cellular Matrix Multiplex Protein labbeling : Nucleus Pro Collagen 1 Collagen 1 Fibronectine Hoechst HeLa Hoechst ; EdU NHEK Cell structure : organelles, cytosquelette, Protein analysis Hoechst ; Actin ; BSEP Human hepatocytes Hoechst; βiii-tubulin; mitotracker SH-SY5Y Hoechst ; AQP3 NHEK Hoechst ; 53BP1 ; γh2ax NHEK Stress : ROS, mitochondrial potential, inflammation Hoechst ; ROS ; mitoctracker NHEK Hoechst ; NFkB human fibroblast + TGFb

Anti-Aging Activity In vitro collagen deposition and fibrosis Fibrosis is involve in wound healing mechanism and represents a major global disease burden. The formation of insoluble pericellular collagen matrix is linked to fibrotic processes and could be assess in vitro for screening procedures prior to animal testing. To improve collagen deposition in vitro, we use charged macromolecules to increase collagen nucleation lead to a granular deposition on human primary fibroblast. This approach is based on the creation of the excluded volume effect (Lareu et al, 2007). Requirements Compounds: pure or extracts Cells: Human Fibroblasts Plates : 96-well plates Time of exposure: 1 day to 1 week Matrix endpoitns : Pro collagen 1 Collagen 1 Fibronectin Imaging and quantifying pericellular matrix In vitro imaging of pericellular matrix required a multiplex protein labbeling for fluorescence high content imaging using our Micro XLS ImageXpress (Molecular Devices). After 5 days of exposure to L- Ascorbic Acid 2-Phosphate Sesquimagnesium (ASC), pericellular matrix was labbeled and quantified. Control The amount of Pro Collagen 1, Collagen 1 and Fibronectin was quantified per cells and compared to control condition (CTL). Thought this model pro and anti fibrotic compounds can be evaluated during several days. Control + NAC Human fibroblast after 5 days of culture Multiplex protein labbeling : Nucleus Pro Collagen 1 Collagen 1 Fibronectine

Anti Inflammatory activity Study inflammation & soothing pathways NFkB (Nuclear Factor kappa-light-chain-enhancer of activated B cells) is found in almost all animal cell types and is a key player in the inflammatory response. It belongs to the category of rapidacting primary transcription factors since it is present in cells in an inactive state, and is quickly activated and is a first responder to harmful cellular stimuli, including pro-inflammatory stimuli. Requirements Compounds: pure or extract Cells: - adherent cells - primary cells or cell line Plates : 96 or 384 wells plates Example of LPS Primary human fibroblasts cells were exposed to several concentrations of bacterial lipopolysaccharide (LPS). Cytosol Pro-inflammatory stimulus Nucleus The nuclear receptor NFkB (green) is translocated from the cytosol into the nucleus -LPS +LPS Primary human dermal fibroblasts: Nuclei in blue, NFkB in green Quantification of nuclear translocation of NFkB after exposure of primary human dermal fibroblasts to increasing concentrations of LPS

Anti-Oxidant Activity Synthesis and storage of Glutathion Glutathione (GSH) is the major antioxidant endogenous peptide, which scavenges reactive oxygen species (ROS) including H2O2. GSH is also involved in detoxifying processes by binding heavy metals, forming water soluble conjugates. Endogenous GSH pool reduction is a cause of oxidative stress damages associated with mitochondrial deterioration. Monochlorobimane reacts with GSH to form a highly fluorescent dye. Requirements Compounds: pure or extracts Time of exposure: 1 day to 1 week Cells: Primary cells and cell line Plates : 96-well plates Endpoints: Glutathion pool % of positive to GSH Cell viability Imaging and quantifying Glutathion Quantifying glutathion (GSH) pool is a marker of anti oxydative properties of compounds. To defined is compounds enhance a curative nor protective effetc, we compared the GSH pool with a oxydative species inducer Menadione (MEN), and GSH inducer N-Acetyl-Cystein (NAC). Control NHEK : Normal Human Epidermal Keratinocytes (NHEK) isolated form juvenile foreskin. HaCaT : Immortal keratinocyte cell line from adult human skin. Control + NAC NAC = N Acetyl Cystein ; MEN = Menadione

Cicatrisation / Repair Assessment Following in vitro wound reparation Wounds can exhibit impaired healing, as a consequence of pathologic failure to process one of the normal stage of healing. Wound healing impairment could be characteristic of the treatments of chronic wounds due to immobilization, diabetes, and skin infection. Characterization of compounds efficacy on wound healing parameters is important dermato/cosmetology, including scar elimination, anti-aging and aesthetic cosmetics and much more. Requirements Compounds: pure or extracts Cells: - keratinocytes - fibroblasts - adherent primary cells or cell line Plates : 96-well plates Scratch : Siclone ALH 3000 96-well head Automated 96-well scratch assay Mechanical scratch is performed using a 96- well head on the whole plate. Cells wound healing is followed in live cells and healed surface is quantified using automated image analysis. Depending on studies objectives, co factors and vitamin C can be used as positive control. Delivered parameters : Percent of healed surface Cell tracking Live recording of cell migration

Oxidative stress assessment Antioxidant protection on primary human keratinocytes NAC = N-acetylcystein Menadione Menadione+ NAC Ctrl + 0,5% DMSO ROS (Inducing Factor) 1,99 1,42 1 NAC protecting factor = 57,7% 100 µm Menadione alone or with 50 µm N acetylcystein, n = 6 ROS = Reactive Oxygen Species Available on all of our cell lines!

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