Stimulated emission depletion-based raster image correlation spectroscopy reveals biomolecular dynamics in live cells

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作者
Per Niklas Hedde
René M. Dörlich
Rosmarie Blomley
Dietmar Gradl
Emmanuel Oppong
Andrew C.B. Cato
G. Ulrich Nienhaus
机构
[1] Institute of Applied Physics and Center for Functional Nanostructures,Department of Cell and Developmental Biology
[2] Karlsruhe Institute of Technology,Department of Physics
[3] Zoological Institute,undefined
[4] Karlsruhe Institute of Technology,undefined
[5] Institute of Toxicology and Genetics,undefined
[6] Karlsruhe Institute of Technology,undefined
[7] University of Illinois at Urbana-Champaign,undefined
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Raster image correlation spectroscopy is a powerful tool to study fast molecular dynamics such as protein diffusion or receptor–ligand interactions inside living cells and tissues. By analysing spatio-temporal correlations of fluorescence intensity fluctuations from raster-scanned microscopy images, molecular motions can be revealed in a spatially resolved manner. Because of the diffraction-limited optical resolution, however, conventional raster image correlation spectroscopy can only distinguish larger regions of interest and requires low fluorophore concentrations in the nanomolar range. Here, to overcome these limitations, we combine raster image correlation spectroscopy with stimulated emission depletion microscopy. With imaging experiments on model membranes and live cells, we show that stimulated emission depletion-raster image correlation spectroscopy offers an enhanced multiplexing capability because of the enhanced spatial resolution as well as access to 10–100 times higher fluorophore concentrations.
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