Quantitative Determination of Dark Chromophore Population Explains the Apparent Low Quantum Yield of Red Fluorescent Proteins.

J Phys Chem B

Nanobiophysics (NBP), MESA+ Institute for Nanotechnology and Technical Medical Centre, Faculty of Science and Technology , University of Twente, PO Box 217, 7500 AE Enschede , The Netherlands.

Published: February 2020

AI Article Synopsis

  • The study investigates the fluorescence quantum yields of four red fluorescent proteins (mCherry, mKate2, mRuby2, and mScarlet) by measuring excited state lifetimes near a gold mirror to control the local density of optical states.
  • The analysis reveals the bright state quantum yield of these proteins is significantly higher than previous reports, emphasizing that mCherry, mKate2, and mRuby2 have up to 45% dark chromophores.
  • In contrast, mScarlet shows a much lower dark fraction (14%) and a high bright state quantum yield of 81%, suggesting that reducing dark chromophores is crucial for optimizing red fluorescent proteins in various applications.

Article Abstract

The fluorescence quantum yield of four representative red fluorescent proteins mCherry, mKate2, mRuby2, and the recently introduced mScarlet was investigated. The excited state lifetimes were measured as a function of the distance to a gold mirror in order to control the local density of optical states (LDOS). By analyzing the total emission rates as a function of the LDOS, we obtain separately the emission rate and the nonradiative rate of the bright states. We thus obtain for the first time the bright state quantum yield of the proteins without interference from dark, nonemitting states. The bright state quantum yields are considerably higher than previously reported quantum yields that average over both bright and dark states. We determine that mCherry, mKate2, and mRuby2 have a considerable fraction of dark chromophores up to 45%, which explains both the low measured quantum yields of red emitting proteins reported in the literature and the difficulties in developing high quantum yield variants of such proteins. For the recently developed bright mScarlet, we find a much smaller dark fraction of 14%, accompanied by a very high quantum yield of the bright state of 81%. The presence of a considerable fraction of dark chromophores has implications for numerous applications of fluorescent proteins, ranging from quantitative fluorescence microscopy to FRET studies to monitoring protein expression levels. We recommend that future optimization of red fluorescent proteins should pay more attention to minimizing the fraction of dark proteins.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7049984PMC
http://dx.doi.org/10.1021/acs.jpcb.9b10396DOI Listing

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