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M Millington, G J Grindlay, K Altenbach, R K Neely, W Kolch, M Bencina, N D Read, A C Jones, D TF Dryden, and S W Magennis (2007)

High-precision FLIM-FRET in fixed and living cells reveals heterogeneity in a simple cfp-yfp fusion protein

Biophysical Chem. 127:155–164.

We have used widefield photon-counting FLIM to study FRET in fixed and living cells using control FRET pairs. We have studied fixed mammalian cells expressing either cyan fluorescent protein (CFP) or a fusion of CFP and yellow fluorescent protein (YFP), and living fungal cells expressing either Cerulean or a Cerulean-Venus fusion protein. We have found the fluorescence behaviour to be essentially identical in the mammalian and fungal cells. Importantly, the high- precision FLIM data is able to reproducibly resolve multiple fluorescence decays, thereby