Absolute quantum yield measurements of fluorescent proteins using a plasmonic nanocavity

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作者
Daja Ruhlandt
Martin Andresen
Nickels Jensen
Ingo Gregor
Stefan Jakobs
Jörg Enderlein
Alexey I. Chizhik
机构
[1] Third Institute of Physics - Biophysics,Georg
[2] Max Planck Institute for Biophysical Chemistry,August
[3] University of Göttingen Medical Faculty,University Göttingen
[4] Clinic of Neurology,Department of NanoBiophotonics
[5] University of Göttingen,Cluster of Excellence “Multiscale Bioimaging: from Molecular Machines to Networks of Excitable Cells,” (MBExC)
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Communications Biology | / 3卷
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摘要
One of the key photophysical properties of fluorescent proteins that is most difficult to measure is the quantum yield. It describes how efficiently a fluorophore converts absorbed light into fluorescence. Its measurement using conventional methods become particularly problematic when it is unknown how many of the proposedly fluorescent molecules of a sample are indeed fluorescent (for example due to incomplete maturation, or the presence of photophysical dark states). Here, we use a plasmonic nanocavity-based method to measure absolute quantum yield values of commonly used fluorescent proteins. The method is calibration-free, does not require knowledge about maturation or potential dark states, and works on minute amounts of sample. The insensitivity of the nanocavity-based method to the presence of non-luminescent species allowed us to measure precisely the quantum yield of photo-switchable proteins in their on-state and to analyze the origin of the residual fluorescence of protein ensembles switched to the dark state.
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