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    • Academia
      Explore BioLegend

      Learn about our world class antibodies for a diverse set of research areas including immunology, neuroscience, cancer, stem cells and cell biology.

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  • Products
    • Research & Development
      • Genomic Analysis
        • IncRNA in Functional Studies
        • Nucleic Acid Isolation
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        • Microplate Readers
        • Microfluidic Nucleic Acid Analysis
        • CRISPR Technologies
        • RNA Interference
        • Transfection and Ancillary Reagents
        • Oligonucleotide Custom Synthesis
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      • Protein Analysis
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        • Sample Dissociation
        • M-PVA Magnetic Beads
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      • Cell Analysis
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      • Research Solutions
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        • Biologics
        • Small Molecule Drug Discovery
        • Disease Research
        • Target Class
        • Drug Development
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        • Functional Genomic Screening Solutions
        • Assay Development Workflows
        • Physiological Model Solutions
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    • Clinical & Diagnostics
      • Reproductive Health
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        • Newborn Screening
        • Newborn Sequencing Research
        • Pregnancy-Relevant Infections
        • Endocrine Reproductive
        • Cell-free DNA Analysis
        • Neonatal Research
        • Preimplantation Genetic Testing
        • PlGF Testing Research
        • Molecular Cytogenetics
        New IVD Mimix™ reference standards for oncology workflows.

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      • Infectious Diseases
        • Tuberculosis Management
        • EUROIMMUN Solutions
        • IDS Solutions
        • Nucleic Acid Isolation for Pathogen Detection
        • Cytomegalovirus
        • SARS-COV-2 Testing Solutions
        • Bacterial & Viral Nucleic Acid Isolation
        • Metagenomics
        New IVD Mimix™ reference standards for oncology workflows.

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      • Cancer
        • ASR Flow Cytometry Antibodies
        • HPV Testing
        • ctDNA Workflows
        • miRNA-seq Analysis
        • Exosome/cfRNA Analysis
        • Targeted Sequencing
        • Mimix Reference Standards
        • Functional Testing
        NEW! Mimix IVD reference standards

        Providing diagnostic labs with trusted quality controls for developing tests and monitoring workflows, with the added assurance of IVD marking. Explore our newest MimixTM controls.

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      • Autoimmunity
        • EUROIMMUN Solutions
        • IDS Solutions
        New IVD Mimix™ reference standards for oncology workflows.

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      • Endocrinology
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      • Allergy
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      • Neurodegeneration
        • Alzheimer's Disease
        • Amytrophic Lateral Sclerosis (ALS)
        • Neurogranin
        • BACE1
        New IVD Mimix™ reference standards for oncology workflows.

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      • Rapid Patient Testing
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      New IVD Mimix™ reference standards for oncology workflows.

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    • Reagents
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      • chemagic Nucleic Acid Purification Kits
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      • CRISPR Technologies
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      • qPCR
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    • Platforms & Automation
      • Nucleic Acid Purification
        • chemagic Applications
        • chemagic IVD Instruments
        • chemagic IVD Kits
        • chemagic Instruments
        • chemagic Kits
        • M-PVA Magnetic Beads
        New! Cellometer™ Ascend™

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      • Automated Liquid Handling
        • Flow Cytometry Cocktail Prep Automation
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        • Automated Liquid Handling Applications
        • Liquid Handling Consumables & Accessories
        New! Cellometer™ Ascend™

        Explore our cell counting and image cytometry solutions.

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      • Integrated Lab Automation
        • Automated Plate Loading
        • Workstation Modules
        • Scheduling & Control Software
        • Robotics
        New! Cellometer™ Ascend™

        Explore our cell counting and image cytometry solutions.

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      • Microfluidic Analysis
        • Microfluidic Protein Characterization
        • Microfluidic Nucleic Acid Analysis
        New! Cellometer™ Ascend™

        Explore our cell counting and image cytometry solutions.

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      • Detection Solutions
        • Plate Reader Accessories
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        • Radiometric Detectors
        • Radiochemicals
        • Liquid Scintillation Cocktails
        • Radiometric Consumables & Accessories
        New! Cellometer™ Ascend™

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      • Imaging
        • Cellular Imaging & Analysis
        • In Vivo Imaging
        New! Cellometer™ Ascend™

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      • Cell Counting and Image Cytometry
        New! Cellometer™ Ascend™

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      • Sample Homogenization
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        • Sample Centrifugation
        • Sample Sonication
        New! Cellometer™ Ascend™

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      • In Vitro Diagnostics (IVD) Platforms & Automation
        • IVD Nucleic Acid Isolation
        • IVD Automated Liquid Handling
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        • EUROIMMUN Instruments
        • IDS Instruments
        • Clinical Applications
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      • Consumables & Accessories
        • Cassettes
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        New! Cellometer™ Ascend™

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      • Instrument Service & Maintenance
        • On Demand Equipment Service
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      New! Cellometer™ Ascend™

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    • Consumables & Accessories
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    • Signals Software
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      • All Solutions
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  • Services
    • Preclinical Services
      • Antibody Drug Conjugate Services
        Preclinical services

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      • Complex Cell Model Screening Services
        Preclinical services

        Work with our experienced scientific team and leverage our advanced technologies to help accelerate the preclinical drug discovery process.

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      • Base Editing Platform
        • Pin-point base editing platform cell line engineering services
        • Pin-point base editing platform pooled tiled screening services
        Preclinical services

        Work with our experienced scientific team and leverage our advanced technologies to help accelerate the preclinical drug discovery process.

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      • Immune Cell Screening
        Preclinical services

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      • Functional Genomic Screening Services
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      • Cell Panel Screening
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      • Cell Line Engineering
        • CHOSOURCE CLE Services
        Preclinical services

        Work with our experienced scientific team and leverage our advanced technologies to help accelerate the preclinical drug discovery process.

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      • Viral Vector Engineering and Manufacture
        Preclinical services

        Work with our experienced scientific team and leverage our advanced technologies to help accelerate the preclinical drug discovery process.

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      Preclinical services

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    • Revvity Omics Services
      • Revvity Omics Clinical Services
        • Cytogenomics
        • Global Laboratory Network
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        • Proactive Testing
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        • Specialized and Customized Assays
        • Sponsored Testing Programs
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Revvity Omics Pharma Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    • Clinical & Testing Services
      • Revvity Omics Clinical Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Revvity Omics Pharma Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Cellular and Humoral Immunoassays
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Tuberculosis Testing Services
        • Oxford Diagnostic Laboratories Service Closures
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    • Customization Services
      • Assays and Reagents
        • Assay Development
        • Compound profiling
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Microplate Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Custom Conjugation & Labeling
        • Custom Labeling
        • Small Molecule
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Radiosynthesis and Labeling
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    • Licensing
      • Gene Delivery Licensing
        CHOSOURCE expression platform

        Revvity's expression platform provides an enhanced system for the development and manufacturing of biotherapeutics that can be used in commercial manufacturing applications.

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      • Gene Expression Systems
        • CHOSOURCE Platform
        • AAV Production Platform
        CHOSOURCE expression platform

        Revvity's expression platform provides an enhanced system for the development and manufacturing of biotherapeutics that can be used in commercial manufacturing applications.

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      • Pin-point™ Base Editing Platform
        CHOSOURCE expression platform

        Revvity's expression platform provides an enhanced system for the development and manufacturing of biotherapeutics that can be used in commercial manufacturing applications.

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      • Virus Screening
        CHOSOURCE expression platform

        Revvity's expression platform provides an enhanced system for the development and manufacturing of biotherapeutics that can be used in commercial manufacturing applications.

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      CHOSOURCE expression platform

      Revvity's expression platform provides an enhanced system for the development and manufacturing of biotherapeutics that can be used in commercial manufacturing applications.

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    • Viral Vector Engineering and Manufacture
      • AAV Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Lentivirus Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    • Instrument Service & Maintenance
      • AV Services
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • Equipment Service Plans
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      • On-demand Equipment Service
        T-SPOT.TB testing services.

        Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    • Customer Training
      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    • OEM Solutions
      T-SPOT.TB testing services.

      Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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    T-SPOT.TB testing services.

    Revvity's Oxford Diagnostic Laboratories is a large referral laboratory for tuberculosis testing services based on our T-SPOT technology.

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  • Company
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      Investor Day 2024

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  • Brands
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    • Popular Revvity Product Brands
    • AlphaLISA and SureFire Ultra

    • BioQule NGS

    • chemagic

    • EnVision Nexus

    • Fontus

    • HTRF

    • IVIS

    • LEGENDplex

    • Opera Phenix

    • T-SPOT

    • TotalSeq

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  • Welcome to Revvity: renowned brands and boundless innovation.

    Hearing the word "can't" is our call to action!

    We help scientists, researchers, and clinicians overcome the world's greatest health obstacles.

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    Learn about our world-class antibodies for a diverse set of research areas including immunology, neuroscience, cancer, stem cells and cell biology.

    Visit BioLegend.com

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High Content Screening Assays

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Cell signalling, physiology and function can all be studied using a high-content analysis approach, and Revvity offers a range of solutions to enable you to develop, perform and analyze your cellular assays with ease. Learn more about the many types of phenotypic assays that can be run in a high-content format and find further details in our application notes.


For research use only. Not for use in diagnostic procedures.

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apoptosis.jpg

Apoptosis

Apoptosis assays are a widely used application in High Content Analysis because of their central role in cancer research and immunology.

There are two main pathways for the induction of apoptosis: the death receptor-mediated pathway and the mitochondrial pathway.

Induction of either pathway will result in the activation of caspases, a class of intracellular cysteine proteases which are considered to be the central components of the apoptotic response.

Imaging based analysis of caspase activation, mitochondrial function and nuclear fragmentation are typical high content apoptosis assays.

Apoptosis assays are a widely used application in High Content Analysis because of their central role in cancer research and immunology.

There are two main pathways for the induction of apoptosis: the death receptor-mediated pathway and the mitochondrial pathway.

Induction of either pathway will result in the activation of caspases, a class of intracellular cysteine proteases which are considered to be the central components of the apoptotic response.

Imaging based analysis of caspase activation, mitochondrial function and nuclear fragmentation are typical high content apoptosis assays.

cell cycle.jpg

Cell cycle

Cell cycle assays are applied in early toxicity testing and in screening for anti-cancer agents. One of the most important aspects in anti-cancer treatments is the inhibition of cell proliferation and cell division.

Both events can be analyzed using High Content Screening (HCS) approaches by multiplexing cell cycle-specific cellular events. Examples are BrdU or EdU staining, which detect the S-phase of the cell cycle by incorporating the nucleoside analog Uridine into newly synthesized DNA strands.

There are also well validated protein markers that are associated with certain cell cycle phases. One example is the phosphorylated histone H3 (pHH3), which is a common M-phase marker. DNA histogramming is another basic analysis tool which transfers very well to image based automated analysis of DNA content per cell.

High Content Screening can quantify all the cell cycle analysis readout parameters which are used in flow cytometry, the traditional tool for cell cycle analysis. Cell cycle analysis relies greatly on statistics over a large number of cells so to get reliable data it is essential to acquire multiple image fields per sample combining data from several thousand cells. A large number of cells must be analyzed in a short period of time in order to achieve an acceptable screen throughput.

Cell cycle assays are applied in early toxicity testing and in screening for anti-cancer agents. One of the most important aspects in anti-cancer treatments is the inhibition of cell proliferation and cell division.

Both events can be analyzed using High Content Screening (HCS) approaches by multiplexing cell cycle-specific cellular events. Examples are BrdU or EdU staining, which detect the S-phase of the cell cycle by incorporating the nucleoside analog Uridine into newly synthesized DNA strands.

There are also well validated protein markers that are associated with certain cell cycle phases. One example is the phosphorylated histone H3 (pHH3), which is a common M-phase marker. DNA histogramming is another basic analysis tool which transfers very well to image based automated analysis of DNA content per cell.

High Content Screening can quantify all the cell cycle analysis readout parameters which are used in flow cytometry, the traditional tool for cell cycle analysis. Cell cycle analysis relies greatly on statistics over a large number of cells so to get reliable data it is essential to acquire multiple image fields per sample combining data from several thousand cells. A large number of cells must be analyzed in a short period of time in order to achieve an acceptable screen throughput.

cell differentiation.jpg

Cell differentiation

Cell differentiation is a multi-step procedure associated with the expression of a specific set of cellular markers in each step, for example the progression of a pluripotent stem cell to a progenitor cell and a fully differentiated tissue specific cell type. The morphology of the cell also changes during differentiation.

Cell differentiation is a multi-step procedure associated with the expression of a specific set of cellular markers in each step, for example the progression of a pluripotent stem cell to a progenitor cell and a fully differentiated tissue specific cell type. The morphology of the cell also changes during differentiation.

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Cell migration

Analysis of cell migration is an important phenotypical assay of processes such as tumor metastasis, immune response and wound healing.

There are four different types of cell migration: migration of cells based on a chemical environment (chemotaxis); cell migration within a gradient of chemoattractants (haptotaxis); movement of cells through the vascular endothelium (transmigration), and migration of cells into a wound to close the gap (wound healing).

Most of these assays are compatible with an imaging based readout. Recent strategies have resulted in more advanced cell migration assays that are more accurate, sensitive, convenient and robust, especially in wound healing.

Analysis of cell migration is an important phenotypical assay of processes such as tumor metastasis, immune response and wound healing.

There are four different types of cell migration: migration of cells based on a chemical environment (chemotaxis); cell migration within a gradient of chemoattractants (haptotaxis); movement of cells through the vascular endothelium (transmigration), and migration of cells into a wound to close the gap (wound healing).

Most of these assays are compatible with an imaging based readout. Recent strategies have resulted in more advanced cell migration assays that are more accurate, sensitive, convenient and robust, especially in wound healing.

cell proliferation.jpg

Cell proliferation

Cell proliferation is the increase in cell number as a result of cell growth and division. 

The accurate assessment of cell number and cell proliferation is useful in many high content assays and is a key readout in cytotoxicity and apoptosis applications. Cell proliferation is also a very sensitive indicator of cell stress since it requires intact cell structures and function.

Cell proliferation is the increase in cell number as a result of cell growth and division. 

The accurate assessment of cell number and cell proliferation is useful in many high content assays and is a key readout in cytotoxicity and apoptosis applications. Cell proliferation is also a very sensitive indicator of cell stress since it requires intact cell structures and function.

cell shape.jpg

Cell shape changes

The shape of a cell can change in response to many different stimuli. The rounding up of cells from an attached and spread-out state on a substrate, for example, can be observed when cells are dividing or experiencing toxic effects.

Analysis of cell spreading is relevant to screening for inhibitors of cell adherence to a substrate. Common measures of the cell shape are area, roundness and width to length ratio.

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The shape of a cell can change in response to many different stimuli. The rounding up of cells from an attached and spread-out state on a substrate, for example, can be observed when cells are dividing or experiencing toxic effects.

Analysis of cell spreading is relevant to screening for inhibitors of cell adherence to a substrate. Common measures of the cell shape are area, roundness and width to length ratio.

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cytoskeletal rearrangment.jpg

Cytoskeletal rearrangement

The cytoskeleton, a filamentous network of actin, tubulin and other protein components, is essential for cellular structure, maintenance, intracellular transport, cell division and many other functions.

Cytoskeletal rerarrangements occur in physiological events such as cell movement. Cytoskeletal defects are frequently associated with diseases such as cancer / metastasis and also cytotoxicity.

Image shows untreated cells(upper left) – structured distribution of tubulin with high intensity near the nucleus and decreasing intensity near the plasma membrane. Re-arrangement of tubulin due to treatment with Demecolcin (lower right).

The cytoskeleton, a filamentous network of actin, tubulin and other protein components, is essential for cellular structure, maintenance, intracellular transport, cell division and many other functions.

Cytoskeletal rerarrangements occur in physiological events such as cell movement. Cytoskeletal defects are frequently associated with diseases such as cancer / metastasis and also cytotoxicity.

Image shows untreated cells(upper left) – structured distribution of tubulin with high intensity near the nucleus and decreasing intensity near the plasma membrane. Re-arrangement of tubulin due to treatment with Demecolcin (lower right).

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Cytotoxicity

The ability to measure early indicators of toxicity is an essential part of drug discovery. In vitro cytotoxicity assays involving tissue specific cell cultures are considered as valuable predictors of human drug toxicity. As a primary organ for drug metabolism, the liver is often subject to toxic effects, so in vitro cellular cytotoxicity studies focus on human hepatocytes.

Early and late indicators of in vitro cytotoxicity include plasma membrane integrity, mitochondrial mass and mitochondrial membrane potential, cell number, caspase activation, nuclear swelling and shrinking and DNA fragmentation.

Determining the count of a cell population is a very sensitive indicator of cell stress since cell proliferation requires intact cell structures and function.

Cytotoxicity assays and their desired readout parameters can vary largely, depending on target cells and compound type. Adaptation of the assay with respect to reagent used, parameters to be evaluated, end point, live or fixed cells and number of cells per sample is critical.

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The ability to measure early indicators of toxicity is an essential part of drug discovery. In vitro cytotoxicity assays involving tissue specific cell cultures are considered as valuable predictors of human drug toxicity. As a primary organ for drug metabolism, the liver is often subject to toxic effects, so in vitro cellular cytotoxicity studies focus on human hepatocytes.

Early and late indicators of in vitro cytotoxicity include plasma membrane integrity, mitochondrial mass and mitochondrial membrane potential, cell number, caspase activation, nuclear swelling and shrinking and DNA fragmentation.

Determining the count of a cell population is a very sensitive indicator of cell stress since cell proliferation requires intact cell structures and function.

Cytotoxicity assays and their desired readout parameters can vary largely, depending on target cells and compound type. Adaptation of the assay with respect to reagent used, parameters to be evaluated, end point, live or fixed cells and number of cells per sample is critical.

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Infection

Traditionally an area for flow cytometry, many infection assays have been transferred from flow cytometry to imaging. High content analysis of cellular infection with pathogens encompasses a large number of different processes about which an imaging based readout can provide essential insights.

It starts with monitoring interactions between a pathogen and the cell surface and the entry of the pathogen into the cell. It involves the understanding of cellular signal transduction and transcriptional response to pathogen infection, all the way to real-time monitoring of cell viability during an infection process.

High resolution confocal imaging, as provided by our Opera Phenix® Plus and Operetta® CLS™ instruments, is an essential technology for a number of assays for infectious diseases. It enables 'mix and measure' homogeneous assays without the need for 'wash away' steps greatly simplifying the assay set-up process for high throughput screening, e.g. when adding an excess of labeled antibody. High resolution imaging is essential for distinguishing punctate signals from evenly distributed signals, for example when analyzing association of viral spikes with lipid rafts.

Traditionally an area for flow cytometry, many infection assays have been transferred from flow cytometry to imaging. High content analysis of cellular infection with pathogens encompasses a large number of different processes about which an imaging based readout can provide essential insights.

It starts with monitoring interactions between a pathogen and the cell surface and the entry of the pathogen into the cell. It involves the understanding of cellular signal transduction and transcriptional response to pathogen infection, all the way to real-time monitoring of cell viability during an infection process.

High resolution confocal imaging, as provided by our Opera Phenix® Plus and Operetta® CLS™ instruments, is an essential technology for a number of assays for infectious diseases. It enables 'mix and measure' homogeneous assays without the need for 'wash away' steps greatly simplifying the assay set-up process for high throughput screening, e.g. when adding an excess of labeled antibody. High resolution imaging is essential for distinguishing punctate signals from evenly distributed signals, for example when analyzing association of viral spikes with lipid rafts.

lipid droplet analysis.jpg

Lipid droplet analysis

Image based analysis of lipid droplet formation is used in two application areas: predicting drug toxicity and metabolic diseases.

Predicting drug toxicity is a major concern for drug regulatory agencies. Phospholipidosis, a lipid storage disorder in which excess phospholipids accumulate within cells, can occur as an adverse drug reaction with many cationic amphiphillic drugs. Drug-induced phospholipidosis in hepatocytes causes failure of the liver, kidney and respiratory system. High Content Assays for phospholipidosis, for example by staining intracellular lipid droplets with fluorescent dyes, are used to predict the toxicity of a compound.

Metabolic diseases can cause a variety of disorders such as hepatosteatosis, which is fat deposition in hepatocytes in the liver. These fat deposits can be visualized and analyzed using High Content Analysis. Other factors that contribute to hepatosteatosis include alcohol, drugs and nutritional disorders.

Image shows lipid droplets in cells, visualized using Bodipy 493/503.

Image based analysis of lipid droplet formation is used in two application areas: predicting drug toxicity and metabolic diseases.

Predicting drug toxicity is a major concern for drug regulatory agencies. Phospholipidosis, a lipid storage disorder in which excess phospholipids accumulate within cells, can occur as an adverse drug reaction with many cationic amphiphillic drugs. Drug-induced phospholipidosis in hepatocytes causes failure of the liver, kidney and respiratory system. High Content Assays for phospholipidosis, for example by staining intracellular lipid droplets with fluorescent dyes, are used to predict the toxicity of a compound.

Metabolic diseases can cause a variety of disorders such as hepatosteatosis, which is fat deposition in hepatocytes in the liver. These fat deposits can be visualized and analyzed using High Content Analysis. Other factors that contribute to hepatosteatosis include alcohol, drugs and nutritional disorders.

Image shows lipid droplets in cells, visualized using Bodipy 493/503.

Dev-Bio_NeuritOutgrowth_Tubulin_Operetta_20xNA_non-confocal_CellCarrier384-252x252.png

Neurite outgrowth

Regeneration of neurons represents a promising strategy for drugs targeted against neurodegenerative injuries and disorders such as Alzheimer’s and Parkinson’s disease. The development of new therapies is focused on identifying molecules that affect the differentiation of neurons and neurite outgrowth.

For this purpose automated measurement and analysis of neuronal cells is essential for neuroscience research and drug discovery. Neurotoxicity is another important area where neurite outgrowth analysis is applied.

Image shows impact of NGF on neurite outgrowth of NS-1 cells. Confocal images of control (upper left panel) and NGF treated (lower right panel) NS-1 cells. Hoechst 33342 stained nuclei are shown in blue. α-tubulin was labeled by immunofluorescence with Alexa Fluor® 488 and is shown in green.

Regeneration of neurons represents a promising strategy for drugs targeted against neurodegenerative injuries and disorders such as Alzheimer’s and Parkinson’s disease. The development of new therapies is focused on identifying molecules that affect the differentiation of neurons and neurite outgrowth.

For this purpose automated measurement and analysis of neuronal cells is essential for neuroscience research and drug discovery. Neurotoxicity is another important area where neurite outgrowth analysis is applied.

Image shows impact of NGF on neurite outgrowth of NS-1 cells. Confocal images of control (upper left panel) and NGF treated (lower right panel) NS-1 cells. Hoechst 33342 stained nuclei are shown in blue. α-tubulin was labeled by immunofluorescence with Alexa Fluor® 488 and is shown in green.

Protein Expression - Autophagy control vs. treated-252x252px.jpg

Protein expression

Protein expression can be very easily quantified in High Content Analysis using either fluorescent protein tags or fluorescently labeled antibodies. Expression on the plasma membrane, in the cytosol and in the nucleus can be distinguished by defining the respective cellular regions.

Example of membrane bound marker (upper left), blue – Hoechst 33342 nuclear dye, green – membrane bound receptor labeled by a fluorescent protein. Region of Interest for protein detection (lower right).

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Protein expression can be very easily quantified in High Content Analysis using either fluorescent protein tags or fluorescently labeled antibodies. Expression on the plasma membrane, in the cytosol and in the nucleus can be distinguished by defining the respective cellular regions.

Example of membrane bound marker (upper left), blue – Hoechst 33342 nuclear dye, green – membrane bound receptor labeled by a fluorescent protein. Region of Interest for protein detection (lower right).

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receptor activation.jpg

Receptor activation

There are many image based approaches for studying receptor activation. Binding of fluorescently labeled ligands to the receptors on the plasma membrane, eventually followed by internalization of the ligand-receptor complex is one of them.

A more relevant method of studying receptor activation is to monitor the processes which follow activation of a receptor, such as internalization and endocytosis of activated receptors carrying a fluorescent tag. This produces a more accurate readout with less false positives.

A more relevant method of studying receptor activation is to monitor the processes which follow activation of a receptor, such as internalization and endocytosis of activated receptors carrying a fluorescent tag. This produces a more accurate readout with less false positives.

Another approach is based on signal molecule recruitment to activated receptor complexes. G protein coupled receptor (GPCR) activation, for example, can be studied by the binding of arrestin carrying a fluorescent protein tag followed by the formation of fluorescent clathrin-coated pits at the cell surface or fluorescent clathrin-coated vesicles in the cytoplasm.

One of the earliest structural changes observed in cells in response to many extracellular factors is membrane ruffling: the formation of motile cell surface protrusions containing a meshwork of newly polymerized actin filaments.

It is becoming clear that actin reorganization is an integral part of early signal transduction pathways, and that many signaling molecules interact with the actin cytoskeleton.

There are many image based approaches for studying receptor activation. Binding of fluorescently labeled ligands to the receptors on the plasma membrane, eventually followed by internalization of the ligand-receptor complex is one of them.

A more relevant method of studying receptor activation is to monitor the processes which follow activation of a receptor, such as internalization and endocytosis of activated receptors carrying a fluorescent tag. This produces a more accurate readout with less false positives.

A more relevant method of studying receptor activation is to monitor the processes which follow activation of a receptor, such as internalization and endocytosis of activated receptors carrying a fluorescent tag. This produces a more accurate readout with less false positives.

Another approach is based on signal molecule recruitment to activated receptor complexes. G protein coupled receptor (GPCR) activation, for example, can be studied by the binding of arrestin carrying a fluorescent protein tag followed by the formation of fluorescent clathrin-coated pits at the cell surface or fluorescent clathrin-coated vesicles in the cytoplasm.

One of the earliest structural changes observed in cells in response to many extracellular factors is membrane ruffling: the formation of motile cell surface protrusions containing a meshwork of newly polymerized actin filaments.

It is becoming clear that actin reorganization is an integral part of early signal transduction pathways, and that many signaling molecules interact with the actin cytoskeleton.

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Reporter gene

Reporter gene assays have easily measurable phenotypes that form the basis of sensitive, quantitative and reproducible assays of eukaryotic gene expression and regulation. Specifically, researchers can use reporter genes to characterize the strength of promoters and enhancers, define the role of transcription factors, assess transfection efficiency or the like. Fluorescent proteins are the most common fluorescent probes for imaging-based reporter gene assays.

Reporter gene assays have easily measurable phenotypes that form the basis of sensitive, quantitative and reproducible assays of eukaryotic gene expression and regulation. Specifically, researchers can use reporter genes to characterize the strength of promoters and enhancers, define the role of transcription factors, assess transfection efficiency or the like. Fluorescent proteins are the most common fluorescent probes for imaging-based reporter gene assays.

signaling pathway analysis.jpg

Signalling pathway analysis

Image based High Content Analysis can support all signaling pathway assays which rely on the translocation of a fluorescently labeled signaling molecule. Transcription factor activation, for example, can be monitored based on their translocation from cytosol to nucleus. Many other signaling molecules translocate from the cytosol to receptor complexes at the plasma membrane.

Image based High Content Analysis can support all signaling pathway assays which rely on the translocation of a fluorescently labeled signaling molecule. Transcription factor activation, for example, can be monitored based on their translocation from cytosol to nucleus. Many other signaling molecules translocate from the cytosol to receptor complexes at the plasma membrane.

Transcription factors control vs. treated-252x252px.jpg

Transcription factors

Transcriptional regulation of genes comprises a multistep process. It starts with the activation of one or more transcription factors in the cell cytoplasm, movement of the transcription factor(s) into the nucleus, and binding to its associated DNA consensus sequence, which initiates the transcription of specific genes. This plays an important role in regulating inflammatory and autoimmune responses, cell proliferation and apoptosis.

Activation of transcription factors can be monitored by imaging as a translocation from the cytoplasm to the nucleus using antibodies for the transcription factors or fluorescent protein tags.

Image shows nuclear translocation of NFkB. Color overlay of the nuclear stain image (Hoechst 33342, blue channel) and labeled NFKB antibody (green channel).

Transcriptional regulation of genes comprises a multistep process. It starts with the activation of one or more transcription factors in the cell cytoplasm, movement of the transcription factor(s) into the nucleus, and binding to its associated DNA consensus sequence, which initiates the transcription of specific genes. This plays an important role in regulating inflammatory and autoimmune responses, cell proliferation and apoptosis.

Activation of transcription factors can be monitored by imaging as a translocation from the cytoplasm to the nucleus using antibodies for the transcription factors or fluorescent protein tags.

Image shows nuclear translocation of NFkB. Color overlay of the nuclear stain image (Hoechst 33342, blue channel) and labeled NFKB antibody (green channel).

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Opera Phenix Plus High-Content Screening System
Opera Phenix Plus High-Content Screening System

The Opera Phenix™ Plus high-content imaging system is a premier confocal solution for your most demanding high content applications. Drawing on over 20 years of experience, the Opera Phenix Plus is designed for high-throughput imaging assays, phenotypic screening, assays using complex disease models, such as live cells, primary cells and microtissues, and fast-response assays, such as Ca2+ flux.

Part number: HH14001000
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Operetta CLS High-Content Analysis System
Operetta CLS High-Content Analysis System

Uncover deep biological understanding in your everyday assays and innovative applications with the Operetta CLS™ high-content analysis system. Featuring a unique combination of technologies, the system delivers the speed, sensitivity and resolution you need to reveal fine sub-cellular details, and our simple yet powerful Harmony software, Operetta CLS lets you find even subtle phenotypic changes.

Part number: HH16000020
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PhenoLOGIC
PhenoLOGIC Machine Learning

PhenoLOGIC™ enables biologists using Harmony to train the software to develop the image analysis algorithms. While other systems may require an image analysis expert to create an algorithm, PhenoLOGIC uses proprietary machine-learning technology to make it easy for you to do it on your own. Using a learn-by-example approach, images can be segmented with just a few clicks of the mouse and then tailored algorithms developed quickly and easily.

Part number: HH12000704
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PreciScan Software
PreciScan Intelligent Acquisition

Harness the power of intelligent image acquisition with PreciScan for more efficient high-content imaging and analysis. This optional plug-in for Harmony high-content analysis software enables you to more accurately target your object of interest for significantly reduced acquisition and analysis times, particularly valuable for 3D microtissue and rare event studies.

Part number: HH17000003
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Application Note
Application Note
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3D cell culture workflow solutions

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Technical Note
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3D volumetric analysis of luminal spaces inside cysts or organoids

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3D volumetric and zonal analysis of solid spheroids

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A brand-new modality on the horizon: how targeted protein degradation can address the unmet need in drug discovery and development

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A multiparametric live-cell cytotoxicity analysis using the Operetta High-content Analysis System

The detection of compound cytotoxicity is an essential part of drug discovery. In this work we describe a rapid and flexible image-based live cell approach to study cytotoxicity. Using a fluorophore dye mixture, multiple cellular phenotypic changes were analyzed following a toxic insult. In order to investigate different drug induced cellular responses, human hepatocytes (HepG2 cells) were treated with various compounds.

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Technical Note
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A scalable and reproducible workflow for high-content analysis of cytotoxic effects in RASTRUM 3D cell cultures

Explore our Technical Note unveiling a robust workflow for advanced cytotoxicity analysis in 3D cell cultures. This method addresses challenges in reproducibility, scalability, and imaging accuracy, enhancing drug testing accuracy and physiological relevance. Key Features: Reproducible 3D Models: Learn the precise creation of 3D matrix cultures using the RASTRUM platform, ensuring consistent dimensions independent of cell type or conditions. Tailored Microenvironment: Tailor matrix stiffness and biofunctionalization for physiologically relevant cell models, significantly improving drug-induced cytotoxicity predictions. Imaging Enhancement: Overcome signal attenuation and data volume challenges in 3D cell culture imaging. Utilize water immersion objectives, optical clearing, and precise positioning techniques for optimal high-content image acquisition. For a comprehensive exploration of this innovative workflow and its applications in 3D cytotoxicity analysis, download the complete Technical Note.

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A scalable method to monitor protein levels and localizations in cells

In this case study, we present a novel method developed by researchers at the CeMM Research Center for studying protein levels and localization within cells. Utilizing CRISPR-Cas9-based intron tagging, this scalable approach generates cell pools expressing hundreds of GFP-fusion proteins, enabling comprehensive analysis of cellular responses to perturbations. Through a combination of intron tagging with in situ sequencing, previously unrecognized proteins impacted by treatments are identified, surpassing the limitations of existing high-throughput methods. This approach can be applied to other sets of genes beyond metabolic enzymes and potentially in a genome-wide manner to study protein dynamics at scale.

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A workflow to characterize and benchmark human induced pluripotent stem cells

The UK-based Human Induced Pluripotent Stem Cell Initiative (HipSci) aims to offer the scientific community access to a vast panel of cell lines with thorough characterization and data analysis tools. This case study details a phenotypic screen to characterize human iPSCs on diverse extracellular matrix substrates, and a method for the capture of specific phenotypes emerging upon cell-to-cell contact. This case study describes: How high-content analysis enables image-based phenotyping and the throughput for analysis of hundreds of cell lines. How data analysis tools help understand multiparametric datasets through interactive data visualization and phenotype classification.

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Addressing the challenges in modern biotherapeutic development

Charter a course to biotherapeutic antibody development success The rise of bispecific antibodies for use as groundbreaking therapies continues to grow with more than 100 bispecific antibodies currently in development. This is thanks to their remarkable versatility from having dual binding sites targeting two different epitopes, providing advantages such as reducing resistance issues, increased specificity, and identifying unique combinations of drug targets. However, navigating the intricate challenges of bispecific antibodies is no small feat. That’s why we’ve created this infographic that will aid you on the journey, equipping you with the knowledge to overcome the obstacles along the way and achieve excellence in bispecific antibody development. Learn more about: Stages that make up the bispecific antibody path Challenges and considerations faced in development Various solutions and technologies available For research use only. Not for use in diagnostic procedures.

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Advanced characterization tools for organoid research: Analyzing cell type diversity, morphology, and function

Organoids are 3D, self-assembling structures derived from stem cells which mimic the structural and functional properties of human tissues. They offer unprecedented insights into development, disease mechanisms, and drug responses. However, before utilizing them in disease modelling or drug discovery applications, a thorough characterization is needed to understand their physiological relevance and their limitations to draw robust conclusions from organoid-based experiments. In this literature review, you’ll discover recent publications that highlight advancements in organoid characterization techniques, focusing on: • Analyzing cell type diversity with flow cytometry • Assessing morphology with high-content imaging • Characterizing cell function with multiplex cytokine immunoassays

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An emerging therapeutic modality - RNA carves its path out of the paradigm

RNA-based therapeutics have garnered significant attention in recent years, fueled by the success of the mRNA COVID-19 vaccines. The development of therapeutics for a broad range of other conditions, including monogenic diseases, metabolic disorders, and cancer, are now being made possible due to advances in RNA-mediated genome editing tools and technologies. Considering the growing interest in RNA therapies, our latest article highlights several promising classes of RNA therapeutic, including RNAi, CRISPR, base editing, and mRNA vaccines, as well as the potential to combine RNA technologies with CAR-T.

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Analysis of mitochondrial dynamics in human iPSC-derived neurons using the Operetta CLS High-Content Analysis System

Mitochondrial dynamics are essential for energy conversion and neuron survival. Understanding changes in mitochondrial dynamics is therefore crucial in developing mitochondria-based therapy options for complex pathological conditions such as cancer, neurological disorders, and metabolic syndromes. Fast kinetic live-cell imaging combined with high-content screening represents a promising strategy to quantitatively track these changes in real time and at large scale. This application note demonstrates how to investigate mitochondrial dynamics in human iPSC-derived neurons using the Operetta ® CLS ™ high-content analysis system. Fast frame rate imaging to accurately capture rapid cellular responses Reliable quantification of mitochondrial dynamics in neurons Flexible kinetic acquisition settings for each channel to avoid unnecessary data acquisition

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Analyzing ERK signal transduction in live cells using a FRET-based biosensor

Extracellular signal-regulated kinase (ERK) is a key component in the regulation of embryogenesis, cell differentiation, cell proliferation, and cell death. The ERK signaling pathway is altered in various cancer types and is frequently investigated as a target for therapeutic intervention. This application note describes how a live cell FRET assay to study ERK signaling was performed on the Operetta CLS ™ high-content analysis system. The optimized design of the FRET-based biosensor, the high-quality imaging of the Operetta CLS system and the easy-to-use image analysis tools of the Harmony™ software contribute to the robustness of the high-content assay.

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Whitepaper
Artificial intelligence, machine learning and deep learning: applications in cellular imaging for improved drug discovery productivity

There has been a lot of buzz around artificial intelligence, machine learning and deep learning. Is the reality living up to the hype? In the world of cellular imaging and its application to drug discovery, there is evidence of real progress against some of the critical challenges facing scientists using these technologies. In this white paper, you will learn about: Challenges in cellular imaging and drug discovery that Artificial Intelligence (AI), Machine Learning (ML) and Deep Learning (DL) are helping to overcome How these technologies are used by leading cellular imaging scientists An outlook to how AI, ML and DL in cellular imaging have the potential to further advance drug discovery and improve productivity in the future

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Whitepaper
Whitepaper
Assessing juvenile batten disease on Brain Development in In Vitro 3D organoid models

Neuronal ceroid lipofuscinosis (NCL) is a complex, rare, and fatal disease belonging to a larger group of lysosomal storage disorders that presents with nervous system symptoms. Batten disease – or CLN3 disease – is another name given commonly to Juvenile NCL (JNCL). Dr. Gomez-Giro and her team focused on understanding the neurodevelopmental process of JNCL utilizing healthy hiPSCs introduced with a disease-causing c.1054C→T pathologic variant into the CLN3 gene. Read the whitepaper to find out more about Dr. Gomez-Giro's research.

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Application Note
Application Note
Automated Single Cell Tracking using Operetta

Here, we present a high-content screening application for analyzing the cell migration of NSCLC cells in a live cell assay.

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Case Study
Case Study
B cell selection and therapeutic antibody characterization using the Operetta high content imaging system

This case study illustrates how Revvity’s high-content imaging solutions support the therapeutic antibody development. Two steps in the workflow - the clonal B cell selection and the functional antibody characterization - rely on high-content screening using the Operetta ™ system. The coupling of the Operetta system to a plate::handler workstation allows the running of plates both day and night, further increasing the throughput. In addition, the EnVision ™ multimode plate reader and the JANUS™ Automated Workstation are essential parts of the workflow that contribute to the throughput of the process and can reduce the variability of liquid handling steps.

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Brochure
Brochure
Biologics workflow solutions

Precision biologics are playing an increasingly powerful role as part of therapeutic strategies such as monoclonal antibodies, bispecific and multispecific antibodies, recombinant proteins, vaccines, and targeted next-generation cell and gene therapies. Harnessing large molecules to create safe and effective therapies is a complex and expensive undertaking. So we help scientists like you develop and streamline your entire biologics workflow, helping you overcome the challenges to bringing consistent, high quality, biological medicines to market – faster than ever before. Explore our solutions and technologies that cover areas of: Biomolecular discovery Biologics characterization Investigating immune function Manufacturing and QA/QC Safety and efficacy

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Literature - Publication Review
Literature - Publication Review
Bone morphogenetic protein 8B - a promising therapeutic avenue for NASH treatment

The incidence and prevalence of non-alcoholic fatty liver disease (NAFLD), which is characterized by excessive accumulation of lipids within the liver, is progressively rising due to increasing obesity and metabolic syndrome prevalence. For some individuals, NAFLD can progress to non-alcoholic steatohepatitis (NASH), which can lead to liver cirrhosis and hepatocellular carcinoma (HCC). NASH is poorly understood and therapies to treat the disease are lacking. Michele Vacca, from the University of Cambridge in the UK and colleagues sought to investigate the impact of one member of the TGFß-BMP superfamily, BMP8B, on the progression of NASH. Learn more about their study.

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Whitepaper
Whitepaper
Cell painting - a cellular imaging and machine learning approach to drug discovery

Phenotypic Drug Discovery Re-Imagined Cell Painting is a phenotypic screening method and a powerful application of high-content screening technology which combines cell and computational biology to elucidate the behavior of cells under the influence of perturbagens, such as chemical compounds, drugs, genes, or other entities. Download our white paper to learn about the origins of the Cell Painting technique, its potential impact on the drug discovery paradigm, together with practical hints and tips for success.

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Application Note
Application Note
Cell painting for phenotypic screening

Cell painting is a powerful high-content screening method which combines cell and computational biology to unravel cells’ responses and gain a deeper understanding of the effects of chemical and genetic perturbagens. However, implementation of cell painting is not without its challenges - from choosing a cell model and labeling reagents, to optimizing instrumentation and making sense of the thousands of features that are extracted during data analysis. Download our application note to learn how to: Set up optimal imaging parameters and see the effect of different acquisition modes on compound clustering Easily perform the assay using the dyes provided in the PhenoVue ® cell painting kit Extract and analyze more than 5700 cellular features Visualize multidimensional data using the Signals ™ VitroVivo platform

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Infographic
Infographic
Cell painting: from images to innovation

Cell painting is an imaging-based phenotypic profiling method that measures phenotypic features to characterize the biological responses of cells to chemical and genetic perturbagens. It finds uses in functional genomics, drug discovery, efficacy, toxicity assessment, and in screening for insights into mechanism-of-action. In this infographic, you will learn: What cell painting is, its history, and how it works What you need to get started How to easily perform the assay using our cell painting solutions

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