Figure 1.
Spectral properties of purified CFP variants at neutral pH.
Absorption (dashed lines) and emission (solid lines) spectra were normalized to maximum of the chromophore band. Emission spectra were recorded with excitation at 420 nm.
Table 1.
Photophysical properties of cyan fluorescent proteins.
Figure 2.
Fluorescence lifetime distributions of purified CFP variants at neutral pH.
The distributions are obtained from maximum entropy analysis of the fluorescence decay curves of (A) ECFP, Cerulean and mTurquoise, (B) ECFP and ECFP-T65S and (C) Cerulean and Cerulean-T65S. For each protein, the distribution shown is an average of six independent experiments recorded at pH 7.4 and T = 20°C.
Figure 3.
pH dependence of the fluorescence intensity of purified CFP variants.
Fluorescence intensities were excited at 420 nm and detected at 474 nm (Δλ = 6 nm). Solid lines correspond to the best fits to a sigmoidal analytical model. Experimental data were normalized to 100% maximum of their analytical fits.
Figure 4.
pH dependence of the spectral properties of purified ECFP.
(A) Absorption spectra normalized to unit maximum absorbance, and (B) emission spectra normalized to unit surface. The spectra corresponding to 50% fluorescence intensity loss (pH = pK1/2) is represented by a continuous red line. The absorption spectrum represented by a dashed gray line corresponds to the first acid pH at which a typical denaturated spectrum is observed.
Figure 5.
Synchrotron radiation circular dichroism on purified CFP variants at neutral and acid pHs.
Comparison of the SRCD spectra of ECFP at pH 7.4 (dashed line) and different CFP variants at pH 2.5 (solid lines). The SRCD spectra were recorded at 25°C.
Figure 6.
pH dependence of the average fluorescence lifetime of purified CFP variants.
Average lifetimes were determined at 20°C from integration of the corresponding lifetime distributions. Solid lines are for eye guidance only.
Figure 7.
Reversible photobleaching of purified CFP variants.
(A) Reversible bleaching kinetics performed on agarose beads labeled with purified CFPs. After prior equilibration in the dark, sudden and constant illumination at 0.2 W/cm2 was applied for less than 15 sec, while camera images were taken every 200 ms. Illumination was then stopped, and, after a minimum of 3 min in the dark, a short series of fluorescence images was collected to check for reversibility. Continuous lines are best fits to the model Fnorm = y0+y1t+y2 exp(−t/τRev) (see Text S1). (B) Amplitudes of the reversible photobleaching responses of the CFP variants.
Figure 8.
Alternate configurations of threonine 65 in the crystallographic structures of ECFP.
Amino-acids and water molecules interacting with the residue 65 hydroxyl are shown, according to the structures of Lelimousin et al (2WSN, solid, grey) [40] and Bae et al (1OXD, transparent, red) [39]. Protein structures were aligned along their main chain backbones, water oxygens are shown as spheres and major H-bonds as dashed lines.