Photobleaching Assays (FRAP & FLIP) to Measure Chromatin Protein Dynamics in Living Embryonic Stem Cells

Malka Nissim-Rafinia; Eran Meshorer

doi:10.3791/2696

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Photobleaching Assays (FRAP & FLIP) to Measure Chromatin Protein Dynamics in Living Embryonic Stem Cells

Article DOI: 10.3791/2696-v • 09:18 min • June 29th, 2011

June 29th, 2011 •

Malka Nissim-Rafinia¹, Eran Meshorer¹

¹Department of Genetics, The Alexander Silberman Institute of Life Sciences, The Hebrew University of Jerusalem

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We describe photobleaching methods including Fluorescence Recovery After Photobleaching (FRAP) and Fluorescence Loss In Photobleaching (FLIP) to monitor chromatin protein dynamics in embryonic stem (ES) cells. Chromatin protein dynamics, which is considered to be one of the means to study chromatin plasticity, is enhanced in pluripotent cells.

Photobleaching Assays (FRAP & FLIP) to Measure Chromatin Protein Dynamics in Living Embryonic Stem Cells

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