Conversion of red fluorescent protein into a bright blue probe
Subach, Oksana M. ; Gundorov, Illia S. ; Yoshimura, Masami ; Subach, Fedor V. ; Zhang, Jinghang ; Grunwald, David ; Souslova, Ekaterina A. ; Chudakov, Dmitriy M. ; Verkhusha, Vladislav V.
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Amino Acid Substitution
Color
Fluorescence Resonance Energy Transfer
Genes, Reporter
HeLa Cells
Humans
Luminescent Proteins
Molecular Probes
Molecular Sequence Data
Mutation
Photochemistry
Sequence Alignment
Sequence Homology
Biochemistry
Biochemistry, Biophysics, and Structural Biology
Chemistry
Molecular Biology
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Abstract
We used a red chromophore formation pathway, in which the anionic red chromophore is formed from the neutral blue intermediate, to suggest a rational design strategy to develop blue fluorescent proteins with a tyrosine-based chromophore. The strategy was applied to red fluorescent proteins of the different genetic backgrounds, such as TagRFP, mCherry, HcRed1, M355NA, and mKeima, which all were converted into blue probes. Further improvement of the blue variant of TagRFP by random mutagenesis resulted in an enhanced monomeric protein, mTagBFP, characterized by the substantially higher brightness, the faster chromophore maturation, and the higher pH stability than blue fluorescent proteins with a histidine in the chromophore. The detailed biochemical and photochemical analysis indicates that mTagBFP is the true monomeric protein tag for multicolor and lifetime imaging, as well as the outstanding donor for green fluorescent proteins in Forster resonance energy transfer applications.
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Subach OM, Gundorov IS, Yoshimura M, Subach FV, Zhang J, Grüenwald D, Souslova EA, Chudakov DM, Verkhusha VV. Conversion of red fluorescent protein into a bright blue probe. Chem Biol. 2008 Oct 20;15(10):1116-24. doi:10.1016/j.chembiol.2008.08.006. Link to article on publisher's site
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Notes
At the time of publication, David Grünwald was not yet affiliated with the University of Massachusetts Medical School.