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फ्लो साइटोमेट्री विश्लेषण×कैको-2 कोशिका पारगम्यता परख (Caco-2 Cell Permeability Assay)×पैच-क्लैंप इलेक्ट्रोफिजियोलॉजी×
क्षेत्रऔषध विज्ञानऔषध विज्ञानऔषध विज्ञान
परिवारProcess / pipelineProcess / pipelineProcess / pipeline
उद्भव वर्ष197619891976
प्रवर्तकLeonard HerzenbergIngrid HidalgoErwin Neher and Bert Sakmann
प्रकारcell analysis and sortingabsorption screeningion channel screening
मौलिक स्रोतHerzenberg, L. A., Parks, D., Sahaf, B., Perez, O., Roederer, M., & Herzenberg, L. A. (2002). The history and future of the fluorescence-activated cell sorter and flow cytometry: a view from Stanford. Clinical Chemistry, 48(10), 1819-1827. DOI ↗Hidalgo, I. J., Raub, T. J., & Borchardt, R. T. (1989). Characterization of the human colon carcinoma cell line (Caco-2) as a model system for intestinal epithelial permeability. Gastroenterology, 96(3), 736-749. DOI ↗Neher, E., & Sakmann, B. (1976). Single-channel currents recorded from membrane of denervated frog muscle fibres. Nature, 260(5554), 799-802. DOI ↗
उपनामFACS, fluorescence-activated cell sorting, cell analysisCaco-2 assay, intestinal permeability, ADME screeningpatch clamp, whole-cell recording, ion channel assay
संबंधित333
सारांशFlow cytometry is a laser-based technology for analyzing and sorting individual cells based on fluorescent markers. Developed by Leonard Herzenberg in the 1970s, flow cytometry enables rapid assessment of cell phenotype, drug effects on cell populations, and therapeutic cell characterization in immunology and hematology.The Caco-2 assay is an in vitro model system using human colon carcinoma cell monolayers to screen drug intestinal permeability. Developed by Hidalgo and colleagues in 1989, Caco-2 cells differentiate into an epithelial barrier resembling intestinal mucosa, enabling rapid assessment of drug absorption potential and identification of transporter-mediated transport.Patch-clamp electrophysiology is a technique for measuring ionic currents through ion channels in cell membranes, developed by Neher and Sakmann in 1976. It enables direct observation of single-channel and whole-cell currents at millisecond resolution, making it essential for characterizing drug effects on ion channels and cardiac safety assessment.
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