Takahito Shingae

Highly efficient NIR to NIR upconversion of ZnMoO4:Tm3+,Yb3+ phosphors and their application in biological imaging of deep tumors

ZnMoO4:Tm3+,Yb3+,K+ nano-phosphors with intense NIR to NIR (excitation by 980 nm, emission at ∼800 nm) upconversion were synthesized by a facile hydrothermal method. The nanoparticles were of the order of 200-400 nm. The XRD patterns confirmed a single phase triclinic structure despite doping small amounts of RE3+ and alkali ions. The optimum concentration of Tm3+, Yb3+ and alkali ions were determined to be 0.1 mol%, 10 mol% and 10 mol%, respectively. Besides charge neutrality, the doped K+ ions affected the crystal field symmetry around the Tm3+ ions which increased the f-f transition probabilities of the RE3+ ions, and hence increased the UC intensities. Compared with ZnMoO4:Tm3+,Yb3+, the NIR to NIR upconversion emission intensity of 10 mol% K+ substituted ZnMoO4:Tm3+,Yb3+ nanocrystals increased by 21-fold and can be pumped by less than 1 mW laser power. The brightest ZnMoO4:Tm3+,Yb3+,K+ nano-phosphor was applied for non-invasively visualizing the tumors in nude mice and successfully detected deep tumors in the thigh muscles. So far, this is the first report of oxide based UCNPs used for in vivo NIR-to-NIR biological imaging and opens the door to the possibility of achieving improved features using non-fluoride based UCNPs.

Raman Optical Activity Probing Structural Deformations of the 4-Hydroxycinnamyl Chromophore in Photoactive Yellow Protein.

Many biological cofactors, such as light-absorbing chromophores in photoreceptors, contain a π-electron system and are planar molecules. These cofactors are, however, usually nonplanar within a protein environment, and such structural distortions have been shown to be functionally important. Because the nonplanar structure makes the molecule chiral, Raman optical activity (ROA) provides a wealth of stereochemical information about the structural and conformational details of cofactors. The present study applied a near-infrared excited ROA to photoactive yellow protein, a blue light receptor. We successfully obtained the ROA spectra of the 4-hydroxycinnamyl chromophore embedded in a protein environment. Furthermore, calculations of the ROA spectra utilizing density functional theory provide detailed structural information, such as data on out-of-plane distortions of the chromophore. The structural information obtained from the ROA spectra includes the positions of hydrogen atoms, which are usually not detected in the crystal structures of biological samples.

Experimental Detection of the Intrinsic Difference in Raman Optical Activity of a Photoreceptor Protein under Preresonance and Resonance Conditions

Raman optical activity (ROA) is an advanced technique capable of detecting structural deformations of light-absorbing molecules embedded in chromophoric proteins. Resonance Raman (RR) spectroscopy is widely used to enhance the band intensities. However, theoretical work has predicted that under resonance conditions the ROA spectrum resembles the shape of the RR spectrum. Herein, we use photoactive yellow protein (PYP) to measure the first experimental data on the effect of changing the excitation wavelength on the ROA spectra of a protein. We observe a close similarity between the shape of the RR spectrum and the resonance ROA spectrum of PYP. Furthermore, we experimentally verify the theoretical prediction concerning the ratio of the amplitudes of the ROA and Raman spectra. Our data demonstrate that selecting an appropriate excitation wavelength is a key factor for extracting structural information on a protein active site using ROA spectroscopy.

Spectroscopic ruler for measuring active-site distortions based on Raman optical activity of a hydrogen out-of-plane vibration

Significance Many biological cofactors, including light-absorbing chromophores in photoreceptors, are modulated upon insertion into a protein. The steric contribution can cause structural distortions in the cofactor, and such effects are considered to be crucial for biological function. For example, the out-of-plane distortion of chromophores is a key factor in controlling their absorption spectra. In spite of the functional importance, such structural distortions are difficult to measure experimentally. In this study, we used a unique capability of Raman optical activity (ROA) to address the above-mentioned issue. This study applied ROA spectroscopy to a photoreceptor protein and indicates that a hydrogen out-of-plane ROA band provides a spectroscopic ruler for the out-of-plane distortion of the chromophore that is embedded in a protein environment. Photoactive yellow protein (PYP), from the phototrophic bacterium Halorhodospira halophila, is a small water-soluble photoreceptor protein and contains p-coumaric acid (pCA) as a chromophore. PYP has been an attractive model for studying the physical chemistry of protein active sites. Here, we explore how Raman optical activity (ROA) can be used to extract quantitative information on distortions of the pCA chromophore at the active site in PYP. We use 13C8-pCA to assign an intense signal at 826 cm−1 in the ROA spectrum of PYP to a hydrogen out-of-plane vibration of the ethylenic moiety of the chromophore. Quantum-chemical calculations based on density functional theory demonstrate that the sign of this ROA band reports the direction of the distortion in the dihedral angle about the ethylenic C=C bond, while its amplitude is proportional to the dihedral angle. These results document the ability of ROA to quantify structural deformations of a cofactor molecule embedded in a protein moiety.