Dissecting the contribution of diffusion and interactions to the mobility of nuclear proteins

doi:10.1529/biophysj.105.071241

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BIOPHYSICAL THEORY AND MODELING

Dissecting the contribution of diffusion and interactions to the mobility of nuclear proteins

Joel Beaudouin ¹, Felipe Mora-Bermudez ², Thorsten Klee ², Nathalie Daigle ² and Jan Ellenberg ²^*

¹ DKFZ Heidelberg
² EMBL, Heidelberg

^* To whom correspondence should be addressed. E-mail: jan.ellenberg{at}embl.de.

Submitted on July 22, 2005
Revised on September 24, 2005
Accepted on 28 November 2005

Abstract
Quantitative characterization of protein interactions underphysiological conditions is vital for systems biology. Fluorescencephotobleaching/activation experiments of GFP-tagged proteinsare frequently used for this purpose, but robust analysis methodsto extract physico-chemical parameters from such data are lacking.Here, we implemented a reaction-diffusion model to determinethe contributions of protein interaction and diffusion on fluorescenceredistribution. The model was validated and applied to fivechromatin-interacting proteins probed by photoactivation inliving cells. We found that very transient interactions arecommon for chromatin proteins. Their observed mobility was limitedby the amount of free protein available for diffusion but notby the short residence time of the bound proteins. Individualproteins thus locally scan chromatin for binding sites, ratherthan diffusing globally before rebinding at random nuclear positions.By taking the real cellular geometry and the inhomogeneous distributionof binding sites into account, our model provides a generalframework to analyze the mobility of fluorescently tagged factors.Furthermore, it defines the experimental limitations of fluorescenceperturbation experiments and highlights the need for complementarymethods to measure transient biochemical interactions in livingcells.

Key Words: FRAP, chromatin, interaction kinetics, photoactivation, reaction-diffusion model

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