Two Distinct Fluorescence States of the Ligand-Induced Green Fluorescent Protein UnaG

Yoh Shitashima; Togo Shimozawa; Akiko Kumagai; Atsushi Miyawaki; Toru Asahi

doi:10.1016/j.bpj.2017.10.022

Two Distinct Fluorescence States of the Ligand-Induced Green Fluorescent Protein UnaG

Biophys J. 2017 Dec 19;113(12):2805-2814. doi: 10.1016/j.bpj.2017.10.022.

Authors

Yoh Shitashima¹, Togo Shimozawa², Akiko Kumagai³, Atsushi Miyawaki³, Toru Asahi⁴

Affiliations

¹ Department of Advanced Science and Engineering, Waseda University, Shinjuku-ku, Tokyo, Japan; Laboratory for Cell Function Dynamics, Brain Science Institute, RIKEN, Wako, Saitama, Japan.
² Department of Life Science and Medical Bioscience, Waseda University, Shinjuku-ku, Tokyo, Japan. Electronic address: togo.shimozawa@gmail.com.
³ Laboratory for Cell Function Dynamics, Brain Science Institute, RIKEN, Wako, Saitama, Japan.
⁴ Department of Advanced Science and Engineering, Waseda University, Shinjuku-ku, Tokyo, Japan; Department of Life Science and Medical Bioscience, Waseda University, Shinjuku-ku, Tokyo, Japan.

Abstract

UnaG is a recently discovered ligand-induced fluorescent protein that utilizes bound bilirubin (BR) as its fluorophore. The fluorescence of the UnaG-BR complex (holoUnaG) compares in quantum efficiency to that of enhanced green fluorescent protein, but it is superior in that the fluorophore formation is instantaneous and not dependent on oxygen; hence, much attention has been paid to UnaG as a new fluorescent probe. However, many important molecular properties of fluorescent probes remain unknown, such as the association/dissociation rates of BR, which determine the stability thereof, and the dispersibility of UnaG in aqueous solutions, which influence the functions of labeled proteins. In this study, we found, in the process of investigating the association rate, that the holoUnaG takes two distinct fluorescence states, which we named holoUnaG₁ and holoUnaG₂. The holoUnaG₁ initially forms after binding BR and then changes to the brighter holoUnaG₂ by a reversible intra-molecular reaction, thereby finally reaching an equilibrium between the two states. Spectroscopic analysis indicated that the intra-molecular reaction was associated not with a chemical change of BR but with a change in the environmental conditions surrounding BR. We also revealed that the molecular brightness ratio and equilibrium population ratio of the two states (holoUnaG₁/holoUnaG₂) were 1:3.9 and 6:4, respectively, using photon number counting analysis. From these results, we have suggested a novel schema, to our knowledge, for the formation of the UnaG and BR complex system and have determined the various rate constants associated therein. Additionally, using analytical ultracentrifugation, we established that UnaG in the apo-state (apoUnaG) and the holoUnaG are monomeric in aqueous solution. These findings provide not only key information for the practical use of UnaG as a fluorescent probe, but also the possibility for development of a brighter UnaG mutant by genetic engineering to constitutive holoUnaG₂.

MeSH terms

Apoproteins / chemistry
Apoproteins / metabolism
Bilirubin / metabolism*
Dose-Response Relationship, Drug
Green Fluorescent Proteins / chemistry*
Green Fluorescent Proteins / metabolism*
Ligands
Sodium Chloride / pharmacology
Spectrometry, Fluorescence
Water / chemistry

Substances

Apoproteins
Ligands
Water
Green Fluorescent Proteins
Sodium Chloride
Bilirubin