Issue 80, 2017

Multicolor protein FRET with tryptophan, selective coumarin-cysteine labeling, and genetic acridonylalanine encoding

Abstract

Site-specific fluorescence probes can be used to measure distances within proteins when used as part of a Förster resonance energy transfer (FRET) pair. Here we report the synthesis of a coumarin maleimide (Mcm-Mal) that is fluorogenic upon reaction with cysteine. We demonstrate that cysteine, acridonylalanine (Acd) double mutant proteins can be produced by unnatural amino acid mutagenesis and reacted with Mcm-Mal to generate Mcm/Acd labeled proteins for FRET studies. The Mcm/Acd FRET pair is minimally-perturbing, easy to install, and well-suited to studying protein distances in the 15–40 Å range. Furthermore, Mcm/Acd labeling can be combined with tryptophan fluorescence in three color FRET to monitor multiple interactions in one experiment.

Graphical abstract: Multicolor protein FRET with tryptophan, selective coumarin-cysteine labeling, and genetic acridonylalanine encoding

Supplementary files

Article information

Article type
Communication
Submitted
15 Jul 2017
Accepted
20 Sep 2017
First published
26 Sep 2017

Chem. Commun., 2017,53, 11072-11075

Multicolor protein FRET with tryptophan, selective coumarin-cysteine labeling, and genetic acridonylalanine encoding

J. J. Ferrie, N. Ieda, C. M. Haney, C. R. Walters, I. Sungwienwong, J. Yoon and E. J. Petersson, Chem. Commun., 2017, 53, 11072 DOI: 10.1039/C7CC05492K

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