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Studying IDP Stability and Dynamics by Fast Relaxation Imaging in Living Cells.

Methods Mol Biol.. 2012;  895:101 - 11
Dhar A, Prigozhin M, Gelman H, Gruebele M. Department of Chemistry, University of Illinois, Urbana-Champaign, IL, USA.
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摘要

Fast relaxation imaging (FReI) temperature-tunes living cells and applies small temperature jumps to them, to monitor biomolecular stability and kinetics in vivo. The folding or aggregation state of a target protein is monitored by Förster resonance energy transfer (FRET). Intrinsically disordered proteins near the structured-unstructured boundary are particularly sensitive to their environment. We describe, using the IDP α-synuclein as an example, how FReI can be used to measure IDP stability and folding inside the cell.

关键词

Temperature jump; Fluorescence; In vivo; Intrinsically disordered protein; Thermal denaturation; Folding kinetics; Folding thermodynamics
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