Kazutaka Hirakawa

Dynamics of singlet oxygen generation by DNA-binding photosensitizers.

The dynamics of photosensitized singlet oxygen generation in a DNA microenvironment were examined using the DNA-binding photosensitizers berberine and palmatine. These photosensitizers generate singlet oxygen only under interaction with DNA because the singlet excited state deactivates rapidly in a nonbinding environment. A kinetic study demonstrated the reaction process whereby singlet oxygen is generated through energy transfer from the triplet excited state of DNA-binding berberine (or palmatine) to molecular oxygen. The guanine-containing sequence of DNA slightly deactivated the singlet excited state of the photosensitizers, resulting in a decrease of the singlet oxygen yield. By the steric hindrance of the DNA strand, the rate constant of the singlet oxygen generation became smaller than that of the other water-soluble photosensitizer.

Singlet Oxygen Generating Activity of an Electron Donor Connecting Porphyrin Photosensitizer Can Be Controlled by DNA

To control the activity of singlet oxygen ((1)O2) generation by photosensitizer through interaction with DNA, the electron- donor-connecting water-soluble porphyrin, meso-(9-anthryl)tris(N-methyl-p-pyridinio)porphyrin (AnTMPyP), was designed and synthesized. Molecular orbital calculation speculated that the photoexcited state of AnTMPyP can be deactivated via intramolecular electron transfer from the anthracene moiety to the porphyrin moiety, forming a charge-transfer (CT) state. The electrostatic interaction between the cationic porphyrin and anionic DNA predicts a rise in the CT state energy, leading to the inhibition of the electron transfer quenching. AnTMPyP showed almost no fluorescence in an aqueous solution, and the fluorescence lifetime was very short (<0.04 ns). Furthermore, this porphyrin did not demonstrate (1)O2 generating activity under photoirradiation. The fluorescence intensity and lifetime of AnTMPyP were markedly increased in the presence of DNA. The photosensitized (1)O2 generation by this porphyrin was also enhanced through interaction with DNA. The estimated quantum yield of (1)O2 generation by AnTMPyP interacting with DNA without guanine sequence was 0.22. The molecular design to control the photosensitized (1)O2 generation is possible based on the regulation of electron transition and steric hindrance of photosensitizing molecule.

Photosensitized protein damage by dimethoxyphosphorus(V) tetraphenylporphyrin

For the purpose of the basic study of photodynamic therapy, the activity of the water-soluble P(V)porphyrin, dimethoxyP(V)tetraphenylporphyrin chloride (DMP(V)TPP), on photosensitized protein damage was examined. The quantum yield of singlet oxygen generation by DMP(V)TPP (0.64) was comparable with that of typical porphyrin photosensitizers. Absorption spectrum measurement demonstrated the binding interaction between DMP(V)TPP and human serum albumin, a water-soluble protein. Photo-irradiated DMP(V)TPP damaged the amino acid residue of human serum albumin, resulting in the decrease of the fluorescence intensity from the tryptophan residue of human serum albumin. A singlet oxygen quencher, sodium azide, could not completely inhibit the damage of human serum albumin, suggesting that the electron transfer mechanism contributes to protein damage as does singlet oxygen generation. The decrease of the fluorescence lifetime of DMP(V)TPP by human serum albumin supported the electron transfer mechanism. The estimated contribution of the electron transfer mechanism is 0.64. These results suggest that the activity of DMP(V)TPP can be preserved under lower oxygen concentration condition such as tumor.

Controlled generation of singlet oxygen by a water-soluble meso-pyrenylporphyrin photosensitizer through interaction with DNA.

An electron donor-connecting water-soluble porphyrin, meso-(1-pyrenyl)-tris(N-methyl-p-pyridinio)porphyrin, did not demonstrate singlet oxygen generating activity under photo-irradiation. The interaction with DNA successfully recovered the photosensitized singlet oxygen generation by this porphyrin.

The molecular mechanism of photochemical internalization of cell penetrating peptide-cargo-photosensitizer conjugates

In many drug delivery strategies, an inefficient transfer of macromolecules such as proteins and nucleic acids to the cytosol often occurs because of their endosomal entrapment. One of the methods to overcome this problem is photochemical internalization, which is achieved using a photosensitizer and light to facilitate the endosomal escape of the macromolecule. In this study, we examined the molecular mechanism of photochemical internalization of cell penetrating peptide-cargo (macromolecule)-photosensitizer conjugates. We measured the photophysical properties of eight dyes (photosensitizer candidates) and determined the respective endosomal escape efficiencies using these dyes. Correlation plots between these factors indicated that the photogenerated 1O2 molecules from photosensitizers were highly related to the endosomal escape efficiencies. The contribution of 1O2 was confirmed using 1O2 quenchers. In addition, time-lapse fluorescence imaging showed that the photoinduced endosomal escape occurred at a few seconds to a few minutes after irradiation (much longer than 1O2 lifetime), and that the pH increased in the endosome prior to the endosomal escape of the macromolecule.

Water-Solubilization of P(V) and Sb(V) Porphyrins and Their Photobiological Application

Porphyrins have been widely utilized as biochemical and biological functional chromophores which can operate under visible-light irradiation. Water-soluble porphyrins have been used as the drug for photodynamic therapy (PDT) and photodynamic inactivation (PDI). Although usual water-solubilization of porphyrins has been achieved by an introduction of an ionic group such as ammonium, pyridinium, sulfonate, phosphonium, or carboxyl to porphyrin ring, we proposed the preparation of water-soluble P and Sb porphyrins by modification of axial ligands. Alkyl (type A), ethylenedioxy (type E), pyridinium (type P), and glucosyl groups (type G) were introduced to axial ligands of Sb and P porphyrins to achieve water-solubilization of Sb porphyrin and P porphyrins. Here, we review their water-soluble P and Sb porphyrins from the standpoints of preparation, bioaffinity, and photosensitized inactivation.

Relaxation Process of Photoexcited meso-Naphthylporphyrins while Interacting with DNA and Singlet Oxygen Generation.

Electron donor-connecting cationic porphyrins meso-(1-naphthyl)-tris(N-methyl-p-pyridinio)porphyrin (1-NapTMPyP) and meso-(2-naphthyl)-tris(N-methyl-p-pyridinio)porphyrin (2-NapTMPyP) were designed and synthesized. DFT calculations speculate that the photoexcited states of 1- and 2-NapTMPyPs can be deactivated via intramolecular electron transfer from the naphthyl moiety to the porphyrin moiety. However, the quenching effect through the intramolecular electron transfer is insufficient, possibly due to the orthogonal position of the electron donor and the porphyrin ring and the relatively small driving force: Gibbs energies are 0.11 and 0.07 eV for 1- and 2-NapTMPyPs, respectively. It was speculated that more than 0.3 eV of the driving force is required to realize effective electron transfer in similar electron-donor connecting porphyrin systems. These porphyrins aggregated around the DNA strand, accelerating the deactivation of their excited singlet state and decreasing their photosensitized singlet oxygen-generating activities. In the presence of a sufficiently large concentration of DNA, these porphyrins can bind to a DNA strand stably, leading to an increased fluorescence quantum yield and lifetime. Singlet oxygen generation was also suppressed by the aggregation of porphyrins around DNA. Although the quantum yield of singlet oxygen generation was recovered in the presence of sufficient DNA, the singlet oxygen generated by DNA-binding porphyrins was significantly smaller than that without DNA. These results suggest that DNA-binding drugs limit the generation of photosensitized singlet oxygen by quenching the DNA strand.

Tetrakis(N-methyl-p-pyridinio)porphyrin and its zinc complex can photosensitize damage of human serum albumin through electron transfer and singlet oxygen generation

The photosensitized protein-damaging activity of water-soluble freebase tetrakis(N-methyl-p-pyridinio)porphyrin (H2TMPyP), and its zinc complex (ZnTMPyP) was investigated using human serum albumin (HSA) as a target protein. These porphyrins bound to HSA and caused photosensitized oxidation of the tryptophan residue. The protein damage was enhanced in deuterium oxide and inhibited by sodium azide, a physical quencher of singlet oxygen, suggesting the contribution of singlet oxygen. However, an excess amount of sodium azide could not completely inhibit protein damage. These findings suggest the partial contribution of another mechanism to the protein damage, possibly the electron transfer mechanism. The Gibbs free energy of the electron transfer mechanism showed that electron transfer-mediated tryptophan oxidation by photoexcited H2TMPyP is more advantageous than that by ZnTMPyP. Actually, the quantum yield of protein damage through electron transfer by H2TMPyP was larger than that by ZnTMPyP. In addition, this study demonstrated that the association between porphyrin and protein plays an important role in photosensitized protein damage.

Photosensitized damage of protein by fluorinated diethoxyphosphorus(V)porphyrin

The effect of the axial ligand fluorination of the water-soluble P(V)porphyrin complex on photosensitized protein damage was examined. The activity of singlet oxygen generation by diethoxyP(V) porphyrin was slightly improved by the fluorination of the ethoxy chains. Absorption spectrum measurements demonstrated the binding interaction between the P(V)porphyrins and human serum albumin, a water-soluble protein. Photo-irradiated P(V)porphyrins damaged the amino acid residue of human serum albumin, resulting in the decrease of the fluorescence intensity from the tryptophan residue of human serum albumin. A singlet oxygen quencher, sodium azide, could not completely inhibit the damage of human serum albumin, suggesting that the electron transfer mechanism contributes to protein damage as does singlet oxygen generation. The decrease of the fluorescence lifetime of P(V)porphyrin by human serum albumin supported the electron transfer mechanism. The estimated contributions of the electron transfer mechanism are 0.57 and 0.44 for the fluorinated and non-fluorinated P(V)porphyrins, respectively. The total quantum yield of the protein photo-oxidation was slightly enhanced by this axial fluorination.

Control of Singlet Oxygen Generation Photosensitized by meso‐Anthrylporphyrin through Interaction with DNA

To control the activity of photosensitized singlet oxygen (1O2) generation, the electron donor‐connecting porphyrin, 5‐(9′‐anthryl)‐10,15,20‐tris(p‐pyridyl)porphyrin (AnTPyP), was designed and synthesized. AnTPyP became water‐soluble by the protonation of the pyridyl moieties in the presence of 5 mm trifluoroacetic acid (pH 2.3). The photoexcited state of the porphyrin ring in an AnTPyP molecule was effectively deactivated by intramolecular electron transfer from the anthracene moiety within 0.04 ns in an aqueous solution. The deactivation was suppressed by the interaction with a DNA strand, resulting in the elongation of the lifetime of the porphyrin excited state and the enhancement of the fluorescence intensity. Furthermore, it was confirmed that the interaction enabled the photoexcited AnTPyP to generate 1O2. Selective 1O2 generation by forming a complex with DNA should be the initial step to realize the target selective photodynamic therapy.