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. 1996 Oct;14(10):1252-6.
doi: 10.1038/nbt1096-1252.

Spatial dynamics of GFP-tagged proteins investigated by local fluorescence enhancement

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Spatial dynamics of GFP-tagged proteins investigated by local fluorescence enhancement

H Yokoe et al. Nat Biotechnol. 1996 Oct.

Abstract

We describe a method of monitoring the spatial dynamics of proteins in intact cells by locally enhancing the blue excited fluorescence of green fluorescent protein (GFP) using a spatially focused ultraviolet-laser pulse. GFP fusion proteins were efficiently expressed by micro-electroporation of in vitro synthesized mRNA into adherent mammalian cells. We found that the diffusion coefficient of cycle 3 mutant GFP was 43 microns2/sec, compared to 4 microns2/sec for wild-type GFP, suggesting that cycle 3 GFP diffuses freely in mammalian cells and is ideally suited as a fusion tag. The local fluorescence enhancement method was used to study the membrane dissociation rate of GFP-tagged K-ras, a small GTP binding protein that localizes to plasma membranes by a farnesyl lipid group and a polybasic region. Our data suggest that K-ras exists in a dynamic equilibrium and rapidly switches between a plasma membrane bound form and a cytosolic form with a plasma membrane dissociation time constant of 1.5 sec.

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  • Cellular probes on the move.
    Simon SM. Simon SM. Nat Biotechnol. 1996 Oct;14(10):1221. doi: 10.1038/nbt1096-1221. Nat Biotechnol. 1996. PMID: 9631080 No abstract available.

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