Two distinct mechanisms of flavoprotein spectral tuning revealed by low‐temperature and time‐dependent spectroscopy

Author:

Nikolaev Andrey1ORCID,Tropina Elena V.23,Boldyrev Kirill N.2,Maksimov Eugene G.4,Borshchevskiy Valentin1,Mishin Alexey1,Yudenko Anna1,Kuzmin Alexander1ORCID,Kuznetsova Elizaveta1,Semenov Oleg1,Remeeva Alina1,Gushchin Ivan1ORCID

Affiliation:

1. Research Center for Molecular Mechanisms of Aging and Age‐Related Diseases Moscow Institute of Physics and Technology Dolgoprudny Russia

2. Institute of Spectroscopy RAS Troitsk Moscow Russia

3. National Research University Higher School of Economics Moscow Russia

4. Faculty of Biology Lomonosov Moscow State University Moscow Russia

Abstract

AbstractFlavins such as flavin mononucleotide or flavin adenine dinucleotide are bound by diverse proteins, yet have very similar spectra when in the oxidized state. Recently, we developed new variants of flavin‐binding protein CagFbFP exhibiting notable blue (Q148V) or red (I52V A85Q) shifts of fluorescence emission maxima. Here, we use time‐resolved and low‐temperature spectroscopy to show that whereas the chromophore environment is static in Q148V, an additional protein‐flavin hydrogen bond is formed upon photoexcitation in the I52V A85Q variant. Consequently, in Q148V, excitation, emission, and phosphorescence spectra are shifted, whereas in I52V A85Q, excitation and low‐temperature phosphorescence spectra are relatively unchanged, while emission spectrum is altered. We also determine the x‐ray structures of the two variants to reveal the flavin environment and complement the spectroscopy data. Our findings illustrate two distinct color‐tuning mechanisms of flavin‐binding proteins and could be helpful for the engineering of new variants with improved optical properties.

Funder

Ministry of Science and Higher Education of the Russian Federation

Russian Science Foundation

Publisher

Wiley

Subject

Molecular Biology,Biochemistry

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