Literature DB >> 10907092

Cell-based, high-content screen for receptor internalization, recycling and intracellular trafficking.

R N Ghosh1, Y T Chen, R DeBiasio, R L DeBiasio, B R Conway, L K Minor, K T Demarest.   

Abstract

A variety of physiologically important receptors are internalized and then recycled back to the plasma membrane by the endocytic recycling compartment. These include the transferrin receptor and many G-protein coupled receptors (GPCRs). The internalization of GPCRs is a result of agonist stimulation. A cell-based fluorescent imaging assay is described that detects and quantifies the presence of fluorescently labeled receptors and macromolecules in the recycling compartment. This High Content Screening application is conducted on the ArrayScan II System that includes fluorescent reagents, imaging instrumentation and the informatics tools necessary to screen for compounds that affect receptor internalization, recycling and GPCR activation. We demonstrate the Receptor Internalization and Trafficking application by quantifying (i) the internalization and recycling of the transferrin receptor using a fluorescently labeled ligand and (ii) the internalization of a physiologically functional model GPCR, a GFP-parathyroid hormone receptor chimera. These assays give high signal-to-noise ratios, broad dynamic ranges between stimulated and unstimulated conditions and low variability across different screening runs. Thus, the Receptor Internalization and Trafficking application, in conjunction with the ArrayScan II System, forms the basis of a robust, information-rich and automated screen for GPCR activation.

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Year:  2000        PMID: 10907092     DOI: 10.2144/00291pf01

Source DB:  PubMed          Journal:  Biotechniques        ISSN: 0736-6205            Impact factor:   1.993


  11 in total

1.  Implementation of high-content assay for inhibitors of mitogen-activated protein kinase phosphatases.

Authors:  Andreas Vogt; John S Lazo
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Review 2.  Neurobiological applications of small molecule screening.

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3.  Exploiting Analysis of Heterogeneity to Increase the Information Content Extracted from Fluorescence Micrographs of Transgenic Zebrafish Embryos.

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Journal:  Assay Drug Dev Technol       Date:  2017-08-11       Impact factor: 1.738

4.  Strategies to Determine Assay Format for the Assessment of Neutralizing Antibody Responses to Biotherapeutics.

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Journal:  AAPS J       Date:  2016-08-05       Impact factor: 4.009

5.  Measuring activity of endocytosis-regulating factors in T-lymphocytes by flow cytometry.

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Journal:  Cytotechnology       Date:  2014-02-07       Impact factor: 2.058

6.  Visualization of human immunodeficiency virus protease inhibition using a novel Förster resonance energy transfer molecular probe.

Authors:  Sha Jin; Erika Ellis; Jithesh V Veetil; Huantong Yao; Kaiming Ye
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7.  A high-content, live-cell, and real-time approach to the quantitation of ligand-induced β-Arrestin2 and Class A/Class B GPCR mobilization.

Authors:  Anthony P Leonard; Kathryn M Appleton; Louis M Luttrell; Yuri K Peterson
Journal:  Microsc Microanal       Date:  2013-01-28       Impact factor: 4.127

Review 8.  Increasing the Content of High-Content Screening: An Overview.

Authors:  Shantanu Singh; Anne E Carpenter; Auguste Genovesio
Journal:  J Biomol Screen       Date:  2014-04-07

9.  Endocytosis as a biological response in receptor pharmacology: evaluation by fluorescence microscopy.

Authors:  Víctor M Campa; Almudena Capilla; María J Varela; Arlet M Acanda de la Rocha; Juan C Fernandez-Troyano; R Belén Barreiro; Juan F Lopez-Gimenez
Journal:  PLoS One       Date:  2015-04-07       Impact factor: 3.240

10.  Evaluating the pharmacological response in fluorescence microscopy images: The Δm algorithm.

Authors:  Ana I Gómez; Marcos Cruz; Juan F López-Giménez
Journal:  PLoS One       Date:  2019-02-13       Impact factor: 3.240

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