QUANTUM YIELDS AND KINETICS OF THE PHOTOBLEACHING OF HEMATOPORPHYRIN, PHOTOFRIN II, TETRA(4-SULFONATOPHENYL)-PORPHINE AND UROPORPHYRIN

Porphyrins used as sensitizers for the photodynamic therapy (PDT) of tumors are progressively destroyed (photobleached) during illumination. If the porphyrin bleaches too rapidly, tumor destruction will not be complete. However, with appropriate sensitizer dosages and bleaching rates, irreversible photodynamic injury to the normal tissues surrounding the tumor, which retain less sensitizer, may be significantly decreased. This paper surveys the quantum yields and kinetics of the photobleaching of four porphyrins: hematoporphyrin (HP), Photofrin II (PF II), tetra(4-sulfonatophenyl)porphine (TSPP) and uroporphyrin I (URO). The initial quantum yields of photobleaching, as measured in pH 7.4 phosphate buffer in air, were: 4.7 x 10(-5), 5.4 x 10(-5), 9.8 x 10(-6), and 2.8 x 10(-5) for HP, PF II, TSPP and URO respectively; thus, the rates of photobleaching are rather slow. Low oxygen concentration (2 microM) significantly reduced the photobleaching yields. However, D2O increased the yields only slightly, and the singlet oxygen quencher, azide, had no effect, even at 0.1 M. Photosensitizing porphyrins in body fluids, cells and tissues may be closely associated with various photooxidizable molecules and electron acceptors and donors. Therefore, selected model compounds in these categories were examined for their effects on porphyrin photobleaching. A number inhibited and/or accelerated photobleaching, depending on the compound, the porphyrin and the reaction conditions. For example, 1.0 mM furfuryl alcohol increased the photobleaching yields of HP and URO more than 5-fold, with little effect on PF II or TSPP. In contrast, the electron acceptor, methyl viologen, increased the photobleaching yield of TSPP more than 10-fold, with little accelerating effect on the other porphyrins. These results suggest that the mechanism(s) of the photobleaching of porphyrin photosensitizers in cells and tissues during PDT may be complex.     

THERMODYNAMICS OF THE BINDING OF HEMATOPORPHYRIN ESTER, A HEMATOPORPHYRIN DERIVATIVE-LIKE PHOTOSENSITIZER, AND ITS COMPONENTS TO HUMAN SERUM ALBUMIN, HUMAN HIGH-DENSITY LIPOPROTEIN AND HUMAN LOW-DENSITY LIPOPROTEIN

The phenomena of the high affinity of porphyrins to the human serum proteins, albumin, high-density lipoproteins (HDL) and low-density lipoproteins (LDL) is well established. Yet, evaluation of the activities of these proteins as endogenous porphyrin carriers, especially with respect to receptor-mediated porphyrin uptake into tumor cells, the merits of which are still in dispute, requires more quantitative protein-porphyrin binding data. As a continuation of previous studies on this issue, the binding of several porphyrin systems to each of the three proteins, employing previously developed spectral methodologies, was studied. The specific systems reported here are hematoporphyrin ester (HPE), which is a novel hematoporphyrin derivative (HPD)-like system, two porphyrin trimers (denoted O1 and O2) and a porphyrin dimer (denoted O3) isolated from HPE. Human serum albumin (HSA) was found to have a single high-affinity site for the monomeric components of HPE, with an equilibrium binding constant of 3.6 × 10⁶. The equilibrium parameters determined for the binding of the three HPE-isolated oligomers to each of the serum proteins are: (1) Binding constants (K_b') of 2.3 × 10⁶, 6.9 × 10⁴ and 1.5 × 10⁴ and number of sites per protein molecule (n) of 3, 1 and 5, for the binding of 01, 02 and 03, respectively, to HSA. (2) K_b’values of 15.5 × 10³, 15.3 × 10³ and 6.6 × 10³ and n values of 1, 2 and 2, for the binding of O1, O2 and O3, respectively, to HDL. (3) K_b’values of 3.3 × 10³, 2.28 × 10⁴ and 8.0 × 10³ and n values of 50, 20 and 16 for the binding of O1, O2 and O3, respectively, to LDL. These data are direct and clear support not only for the high affinity of porphyrins to serum proteins but specifically of stable oligomers that have been assigned critical roles in the photodynamic treatment of tumors. Of the three proteins, LDL is clearly the best camer, providing the highest drug payload with a moderate affinity (enough to bind and not too much to prevent release). These data are suggested to be promising for the postulated role of LDL in porphyrin uptake into tumor cells and to be useful in the future as benchmarks for novel porphyrin systems.     

SITES OF PHOTODYNAMICALLY INDUCED DNA REPAIR IN HUMAN CELLS

Abstract Human REH cells were incubated with the photosensitizers meso -tetra(4-sulfonatophenyl)porphyrin (TSPP=TPPS₄) or meso -tetra(3-hydroxyphenyl)porphyrin (3-THPP). The relatively hydrophilic TSPP was partly found in the cytoplasm and partly in the nuclei, whereas the lipophilic 3-THPP was found apparently in membranes and not inside the nuclei. After illumination, sites of DNA repair were labeled by means of a monoclonal antibody against proliferating cell nuclear antigen (PCNA) bound in the nuclei. The amount of bound PCNA in non-S-phase cells was proportional to the light dose. The bound PCNA was homogeneously distributed in the nuclei 0.5 h after photodynamic treatment (PDT) with TSPP. In contrast, for cells given PDT with 3-THPP, the periphery of the nuclei was selectively labeled, indicating that the initial DNA damage was localized close to the sensitizer at the nuclear membrane.     

PHOTOBLEACHING OF MONO-l-ASPARTYL CHLORIN e6 (NPe6): A CANDIDATE SENSITIZER FOR THE PHOTODYNAMIC THERAPY OF TUMORS

Abstract— Most sensitizers used for the photodynamic therapy (PDT) of tumors photobleach on illumination. Thus, it is of interest to examine the photobleaching behavior of new sensitizers proposed for use in PDT. This report surveys the quantum yields and kinetics of the photobleaching of mono- l -aspartyl chlorin e₆ (NPe6), a hydrophilic chlorin that has many of the photoproperties desirable in a sensitizer for clinical PDT. It is a very effective sensitizer for the PDT of several types of model tumors in animals and is now in Phase I clinical trials. The quantum yield of NPe6 photobleaching in pH 7.4 phosphate buffer in air was 8.2 × 10⁻⁴; this is greater than the yields for typical porphyrin photosensitizers. For example, the yields for hematoporphyrin and uroporphyrin are 4.7 × 10 ⁵ and 2.8 × 10⁻⁵, respectively. The yield decreased significantly in organic solvents of low dielectric constant. The Sn derivative of NPe6 was more light stable than NPe6 (yield = 5.7 × 10 ⁻⁶), while the Zn derivative was more sensitive (yield = 1.9 × 10⁻²). Oxygen appeared to be necessary for the photobleaching of NPe6; however, bleaching was not inhibited by 100 mM azide, an efficient quencher of singlet oxygen. The photooxidizable substrates cysteine, dithiothreitol and furfuryl alcohol increased the quantum yield of photoblcaching two- to four-fold, while the electron acceptor, met-ronidazole, increased it almost six-fold. Photobleaching yields for several other chlorins were also measured.     

THE EFFECTS OF PERIPHERAL SUBSTITUENTS ON THE KINETICS OF ZINC ION INCORPORATION AND ACID CATALYZED REMOVAL FROM WATER SOLUBLE SULFONATED PORPHYRINS

Abstract

The kinetics of Zn²⁺ and Zn(OH)⁺ incorporation into and the kinetics of the acid catalyzed removal of Zn(II) from twelve water-soluble, sulfonated derivatives of tetraphenylporphyrin with alkyl or halogen groups in the para, ortho or di-ortho positions were investigated. While the incorporation reactions showed little dependence on porphyrin basicity, the Zn-P (P = porphyrin derivative) acid solvolysis reactions were faster the higher the basicity of the free base (H₂-P) compound. Equilibrium constants for the formation of cadmium porphyrins decreased with an increase in porphyrin basicity. The predeformed tetrakis(4-sulfonatophenyl)-β-octabromo-porphyrin reacted with Zn²⁺ about 10³ times faster than porphyrins of similar basicity. These results indicate how substituents on the phenyl and beta-pyrrole rings influence the solution chemistry of water soluble porphyrins.     

Measurement of Intracellular Oxygen Concentration During Photodynamic Therapy in vitro

A technique is introduced that monitors the depletion of intracellular ground state oxygen concentration ([³O₂]) during photodynamic therapy of Mat‐LyLu cell monolayers and cell suspensions. The photosensitizer Pd(II) meso‐tetra(4‐carboxyphenyl)porphine (PdT790) is used to manipulate and indicate intracellular [³O₂] in both of the in vitro models. The Stern–Volmer relationship for PdT790 phosphorescence was characterized in suspensions by flowing nitrogen over the suspension while short pulses of 405 nm light were used to excite the sensitizer. The bleaching of sensitizer and the oxygen consumption rate were also measured during continuous exposure of the cell suspension to the 405 nm laser. Photodynamic therapy (PDT) was conducted in both cell suspensions and in cell monolayers under different treatment conditions while the phosphorescence signal was acquired. The intracellular [³O₂] during PDT was calculated by using the measured Stern–Volmer relationship and correcting for sensitizer photobleaching. In addition, the amount of oxygen that was consumed during the treatments was calculated. It was found that even at large oxygen consumption rates, cells remain well oxygenated during PDT of cell suspensions. For monolayer treatments, it was found that intracellular [³O₂] is rapidly depleted over the course of PDT.     

Conductive Fused Porphyrin Tapes on Sensitive Substrates by a Chemical Vapor Deposition Approach

Oxidative polymerization of nickel(II) 5,15‐diphenyl porphyrin and nickel(II) 5,15‐bis(di‐3,5‐tert‐butylphenyl) porphyrin by oxidative chemical vapor deposition (oCVD) yields multiply fused porphyrin oligomers in thin film form. The oCVD technique enables one‐step formation, deposition, and p‐doping of conjugated poly(porphyrins) coatings without solvents or post‐treatments. The decisive reactions and side reactions during the oCVD process are shown by high‐resolution mass spectrometry. Owing to the highly conjugated structure of the fused tapes, the thin films exhibit an electrical conductivity of 3.6×10^?2 S cm^?1 and strong absorption in the visible to near‐infrared spectral region. The formation of smooth conjugated poly(porphyrins) coatings, even on sensitive substrates, is demonstrated by deposition and patterning on glass, silicon, and paper. Formation of conductive poly(porphyrins) thin films could enable the design of new optoelectronic devices using the oCVD approach.     

Aggregation and solution behavior of 5-(1-(4-carboxybutyl) pyridinum-4-yl) 10,15,20-tris (1-methylpyridinium-4-yl) porphyrin: A resonance light scattering, fluorescence and absorption spectroscopic study

Aggregation behavior of water soluble porphyrins, 5-(1-(4-carboxybutyl) pyridinum-4-yl) 10,15,20-tris (1-methylpyridinium-4-yl) porphyrin (5-CBPyP) in the presence of various concentrations of calf thymus DNA (ct-DNA) and sodium chloride were studied in comparison with meso-tetrakis (4-N-methyl pyridinum) porphyrin (TMPyP), by optical absorption, fluorescence and resonance light scattering (RLS) spectroscopies. Both porphyrins obey Beer’s law in extended range of concentration. Optical absorption and RLS measurements demonstrated nonaggregation for both porphyrins under increasing concentration of ct-DNA and NaCl. However, in comparison, 5-CBPyP had less tendency for aggregation that may be taken as an advantage for its probable application in photodynamic therapy of cancer. The trend of changes in absorption spectra of both porphyrins in the presence of ct-DNA indicates the homogeneous intercalation binding mode. The values of (2.81 ± 0.28) × 10⁶ M^?1 and (0.95 ± 0.09) × 10⁶ M^?1 were obtained for apparent binding constant of TMPyP and 5-CBPyP from analysis of optical absorption data, respectively. This indicates the less affinity of 5-CBPyP to ct-DNA in comparison with TMPyP. The binding of both porphyrins to ct-DNA quenches fluorescence emission of Ethidium bromide (EB) that is bound to ct-DNA. The quenching process obeys linear Stern-Volmer relationship indicating the displacement of EB from its binding sites by these porphyrins. The results of this technique also represent the intercalation mode of binding for both porphyrins and higher binding affinity of TMPyP compared with 5-CBPyP.     

Surface-enhanced Raman scattering of TSPP,Ag(II)TSPP,and Pb(II)TSPP adsorbed on AgI and AGCl colloids

Surface-enhanced Raman scattering (SERS) was measured for meso-tetrakis(4-sulfonatophenyl)porphine (TSPP) and its metal derivatives Ag(II)TSPP and Pb(II)TSPP adsorbed on AgI colloids, and for TSPP adsorbed on AgCl colloids. The experiments show that TSPP molecules adsorbed on AgI colloids undergo a silver incorporation, while TSPP adsorbed on AgCl colloids are converted into the porphyrin diacid H₄TSPP²⁺ and the metalloporphyrin Ag(II)TSPP. The concentration dependences of SERS spectra for TSPP adsorbed on the two substrates are quite different.     

Amino Acid–Porphyrin Conjugates: Synthesis and Study of their Photophysical and Metal Ion Recognition Properties

Synthesis, photophysical and metal ion recognition properties of a series of amino acid‐linked free‐base and Zn‐porphyrin derivatives (5–9) are reported. These porphyrin derivatives showed favorable photophysical properties including high molar extinction coefficients (>1 × 10⁵ m ^?1 cm^?1 for the Soret band), quantum yields of triplet excited states (63–94%) and singlet oxygen generation efficiencies (59–91%). Particularly, the Zn‐porphyrin derivatives, 6 and 9 showed higher molar extinction coefficients, decreased fluorescence quantum yields, and higher triplet and singlet oxygen quantum yields compared to the corresponding free‐base porphyrin derivatives. Further, the study of their interactions with various metal ions indicated that the proline‐conjugated Zn‐porphyrins (6 and 9) showed high selectivity toward Cu²⁺ ions and signaled the recognition through changes in fluorescence intensity. Our results provide insights on the role of nature of amino acid and metallation in the design of the porphyrin systems for application as probes and sensitizers.     

Photodynamic studies and photoinactivation of Escherichia coli using meso-substituted cationic porphyrin derivatives with asymmetric charge distribution

The photodynamic activities of novel asymmetrically meso-substituted cationic porphyrins, 5,10-di(4-methylphenyl)-15,20-di(4-trimethylammoniumphenyl)porphyrin iodide 1 and 5-(4-trifluorophenyl)-10,15,20-tris(4-trimethylammoniumphenyl)porphyrin iodide 2 and its metal complex with Pd(II) 3, have been investigated in both homogeneous medium bearing photooxidizable substrates and in vitro on a typical gram-negative bacterium Escherichia coli. The amphiphilic character of porphyrin 2 was increased by the presence of a high-lipophilic trifluoromethyl group and its photophysical properties changed by forming a complex with Pd(II). Absorption and fluorescence spectroscopic studies were compared in different media. Fluorescence quantum yields (phi(F)) of 0.16 for 1 in tetrahydrofuran and 0.08 for 2 in N, N-dimethylformamide (DMF) were calculated, whereas no significant emission was detected for Pd(II) porphyrin 3. The singlet molecular oxygen, O(2)((1)Delta(g)), production was evaluated using 9,10-dimethylanthracene in DMF yielding relative values of 1, 0.55 and 0.47 for porphyrins 3, 2 and 1, respectively. A faster decomposition of l-tryptophan was obtained using Pd(II) porphyrin 3 as sensitizer with respect to the free-base porphyrins 1 and 2. In biological medium, the behavior of cationic porphyrins 1-3 were compared with that of 5-(4-carboxyphenyl)-10,15,20-tris(4-methylphenyl)porphyrin 4, which was used as a noncationic sensitizer. These porphyrins are rapidly bound to E. coli cells in 5 min and the amount of cell-bound sensitizer is not appreciably changed incubating the cultures for longer times. The recovered porphyrin 2 after one washing step reaches a value of approximately 2.9 nmol/10(6) cells and this amount remains high even after three washes, indicating that this sensitizer is tightly bound to cells. Photosensitized inactivation of E. coli was analyzed using cells without and with one washing step. In both cases, a higher photoinactivation of cells was found for tricationic porphyrin 2 and 3, causing a approximately 5.5 log (99.999%) decrease of cell survival, when treated with 10 microM of sensitizer. Under these conditions, a lower effect was found for porphyrin 1 (approximately 4 log) whereas sensitizer 4 did not produce appreciable photodamage. The results were also confirmed by growth delay experiments. These studies show that the amphiphilic tricationic porphyrin 2 and 3 bearing a trifluoromethyl group can be a promising model for phototherapeutic agents with potential applications in inactivation of bacteria by photodynamic therapy.     

In vivo AND PHOTOPHYSICAL STUDIES ON PHOTOOXIDATIVE DAMAGE TO LENS PROTEINS AND THEIR PROTECTION BY RADIOPROTECTORS

Abstract— Photooxidation, whether initiated by an endogenous or exogenous sensitizer, is an important mechanism in light induced damage to the lens. One of the substrates for this damage is lens protein. A porphyrin sensitizer which binds to lens proteins [ mesotetra ( p -sulfonatophenyl) porphyrin (TPPS)] was found to photooxidize Skh-2 pigmented mice lens protein in vivo. Uroporphyrin, a model for a non-binding photosensitizer, did not induce photooxidative damage to the mouse lens.
The radioprotector 3-amino-2-hydroxypropyl phosphorothioate (WR-77913) was investigated as an agent to retard or negate in vivo photooxidative damage to the lens. Intraperitoneal injections of WR-77913 prior to irradiation reduced the TPPS induced photodestruction of lens protein in Skh-2 pigmented mice.
The mechanism of protection was also investigated. Thiols were found to quench both the triplet state of porphyrins and the reactive intermediate singlet oxygen on the order of 10⁵ and 10⁶ M ^-1 s¹ respectively. These are probably not fast enough to explain most of the protection afforded by thiols. An additional mechanism may be the accelerated photobleaching of porphyrins by thiols which protects tissue by reducing the absorptions due to the porphyrins.     

Kinetic studies of a catalyzed metalloporphyrin formation

Kinetics of the incorporation of mercury(II) ion in tetra (p-trimethylammoniumphenyl)porphine have been investigated in aqueous solution at 30.0°C and 0.2 M (NaNO₃) ionic strength. The reaction was found to be first order each in mercury(II) and the porphyrin. The forward (formation) and the reverse (dissociation) rate constants were found to be 1.9 ± 0.2 × 10³ M^?1 s^?1 and 7 ± 2 × 10⁶ M^?1 s^?1, respectively. Kinetics of zinc(II) incorporation in tetra(p-trimethylammoniumphenyl)porphine catalyzed by mercury(II) were also investigated. This catalysis is explained in terms of steady-state formation of mono mercury(II) porphyrin followed by zinc(II) displacement of mercury(II) ion from the porphyrin. Such a mechanism also illustrates the importance of porphyrin core deformation to metal incorporation.     

A New Nonconjugated Naphthalene Derivative of Meso-tetra-(3-hydroxy)-phenyl-porphyrin as a Potential Sensitizer for Photodynamic Therapy

A new 5,10,15,20-tetra-(phenoxy-3-carbonyl-1-amino-naphthyl)-porphyrin was prepared by an isocyanate condensation reaction and its photophysical properties fully evaluated, both in terms of photostability and singlet oxygen production. It shows considerably enhanced photostability when compared with the parent 5,10,15,20-tetra-(3-hydroxy-phenyl)-porphyrin, with the photodegradation quantum yields for T(NAF)PP and T(OH)PP being 4.65 × 10⁻⁴ and 5.19 × 10⁻³, respectively. Its photodynamic effect in human carcinoma HT-29 cells was evaluated. The new porphyrin showed good properties as a sensitizer in photodynamic therapy with an in vitro cytotoxicity IC₅₀ value of 6.80 μg mL⁻¹ for a 24 h incubation. In addition to the potential of this compound, the synthetic route used provides possibilities of extension to a wide range of new sensitizers.     

THE PHOTOEXCITED TRIPLET STATE OF TETRAPHENYL CHLORIN, MAGNESIUM TETRAPHENYL PORPHYRIN AND WHOLE CELLS OF CHLAMYDOMONAS REINHARDI. A LIGHT MODULATION-EPR STUDY

Abstract— The photoexcited triplet states of frozen solutions of tetraphenyl chlorin (TPC), magnesium tetraphenyl porphyrin (MgTPP) and whole cells of Chlamydomonas reinhardi have been studied by light modulation-EPR spectroscopy. The porphyrins were chosen to be studied as model compounds for chlorophyll molecules, From EPR spectra the zero field splitting parameters (ZFS) were calculated. For TPC, |D| = 0.0364 ± 0.0002 cm^-1, |E| = 0.0063 ± 0.0002 cm^-1. For MgTPP, |D| = 0.0310 ± 0.0002 cm^-1. For chloroplasts, |D| = 0.0280 ± 0.0004 cm^-1, |E| = 0.0032 ± 0.0004 cm^-1. In all compounds studied, except MgTPP, electron spin polarization (ESP) was observed. From the analysis of the kinetic curves at each canonical orientation we evaluated the spin lattice relaxation rate W, the depopulation rate constants k_p, and the ratio between the population rate constants, A_p, at zero magnetic field. For TPC in ethanol-toluene (5:1) k_x= (0.70 ± 0.10) × 10³ s^-1, k_y= (0.40 ± 0.07) × 10³ s^-1, k_x= (0.24 ± 0.05) × 10³ s^-1; A_x:A_y:A_z? 1.0:0.6:0.4; W= (2.60 ± 0.40) × 10³ s^-1. For MgTPP, only the total decay rate constant, k_T, was calculated: (1.5 ± 0.2) × 10 s^-1 in n-octane and (4.8 ± 0.8) × 10 s^-1 in ethanol. The results for TPC and MgTPP are compared to those reported previously for chlorophyll. It is concluded that the dynamics of the photoexcited triplet state in chlorophylls are mainly governed by the chlorin macrocycle. From the EPR spectrum and ZFS parameters of chloroplasts, we propose that both chlorophyll a and chlorophyll b are the main constituents of the EPR spectrum. From the analysis of the kinetic curves we obtain separately the kinetic parameters for chlorophylls a and b, k^a_x= (1.30 ± 0.20) × 10³ s^-1, k^a_y;= (0.85 ± 0.15) × 10³ s^-1k^a_x= (0.32 ± 0.05) × 10³ s^-1; A^a_x:A^a_y:A^a_z? 1.0:0.7:0.2; W^a= (1.20 ± 0.20) × 10³ s^-1; k^b_x= (0.56 ± 0.09) × 10³ s^-1, k^b_y= (0.30 ± 0.04) × 10³ s^-1, k^b_z= (0.06 ± 0.01) × 10³ s^-1; A^b_x:A^b_y:A^b_x? 1.0:0.6:0.1; W^b= (5.00 ± 0.80) × 10³ s^-1. These results are very close to those found separately for chlorophyll a and chlorophyll b oligomers in vitro.     

Chlorins as photosensitizers in biology and medicine

The photodynamic therapy (PDT) of tumors involves illumination of the tumorous area following the administration of a tumor-localizing photodynamic sensitizer. Hematoporphyrin derivative (HPD) and Photofrin II (a purified form of HPD), the main sensitizers used clinically for PDT to date, are complex mixtures of porphyrins; furthermore, these preparations absorb light very poorly in the red region of the spectrum (wavelengths greater than 600 nm) where light penetration into mammalian tissues is greatest. Thus there is considerable interest in identifying new sensitizers that localize more effectively in tumors, absorb more strongly at longer wavelengths and can be prepared in high purity. Much of this interest has been directed towards chlorins (reduced porphyrins), which typically absorb strongly in the red. This review summarizes research that has been carried out on selected types of chlorins, some of which may have important applications as sensitizers for PDT.     

A Five‐layer π‐Aromatic Structure Formed through Self‐assembly of a Porphyrin Trimer and Two Aromatic Guests

In this study we synthesized two‐ and four‐armed porphyrins – bearing two carboxyl and four 2‐aminoquinolino functionalities, respectively, at their meso positions – as a complementary hydrogen bonding pair for the self‐assembly of a D₂‐symmetric porphyrin trimer host. Two units of the two‐armed porphyrin and one unit of the four‐armed porphyrin self‐assembled quantitatively into the D₂‐symmetric porphyrin trimer, stabilized through ammidinium‐carboxylate salt bridge formation, in CH₂Cl₂ and CHCl₃. The porphyrin trimer host gradually bound two units of 1,3,5‐trinitrobenzene between the pair of porphyrin units, forming a five‐layer aromatic structure. At temperatures below ?40 °C, the rates of association and dissociation of the complexes were slow on the NMR spectroscopic time scale, allowing the 1 : 1 and 1 : 2 complexes of the trimer host and trinitrobenzene guest(s) to be detected independently when using less than 2 eq of trinitrobenzene. Vis titration experiments revealed the values of K₁ (2.1±0.4×10⁵ M^?1) and K₂ (2.2±0.06×10⁴ M^?1) in CHCl₃ at room temperature.     

CARBON-14 LABELING AND BIOLOGICAL ACTIVITY OF THE TUMOR-LOCALIZING DERIVATIVE OF HEMATOPORPHYRIN

Abstract— Carbon-14-labeled hematoporphyrin ([¹⁴C]HP) was synthesized by two methods, (i) Using an in vitro avian whole-blood system, [¹⁴C]protoheme was obtained biosynthetically by incorporating [⁴C]aminolevulinic acid into the porphyrin ring structure. Subsequently, the [¹⁴C]protoheme was converted to [⁴C]HP by standard procedures, (ii) By adopting several well-characterized chemical reactions, deuteroporphyrin was treated with [¹⁴C]acetyl chloride, giving [¹⁴C]diacetyl deuteroporphy-rin which was readily reduced and hydrolyzed to [¹⁴C]HP (with thecarbon–14 label on the hydroxyethyl side-chains). These two methods are simple and afford good yields of [¹⁴C]HP with moderate to high specific activities. The [¹⁴C]HP was then treated with acetic acid/sulfuric acid followed by sodium hydroxide to give [¹⁴C]HPD. Upon gel- and ultra-filtration, the [¹⁴C]HPD was enriched in the so-called tumor-localizing fraction of HPD, giving [¹⁴C]PII with specific activities of 0.4 Ci/mol (biosynthesis) and 10 Ci/mol (chemical synthesis). These [¹⁴C]PII preparations were equivalent with respect to chromatographic and spectrophotometric characteristics, as well as tumoricidal photodynamic activity in the DBA/2 Ha-DD mouse: SMT-F tumor system, to the unlabeled commercial product Photofrin^? II. The distribution of [¹⁴C]PII in mouse tissues was in close agreement to that previously reported, after adjustment for dose, for [¹⁴C]HPD biosynthetically labeled in vivo (Gomer and Dougherty, 1979), as well as for Photofrin^? II, where tissue levels were determined spectrophotometrically after extraction (Dougherty and Mang, unpublished).     

Effects of pluronic silica nanoparticles on the photophysical and photodynamic therapy behavior of triphenyl-p-phenoxy benzoic acid metalloporphyrins

5, 10, 15, Triphenyl-20-p-phenoxy benzoic acid porphyrins (P) containing Zn (ZnP), Ga (GaP), and Si (SiP) were synthesized and conjugated to pluronic-silica (PluS) nanoparticles (NPs) where the fluorescence and singlet oxygen generating behavior of the porphyrins were investigated. The highest singlet oxygen quantum yield (Φ_Δ) was obtained for ZnP. When the porphyrins were conjugated to the PluS NPs, the Φ_Δ was quenched and fluorescence was enhanced. The pore size of the NPs upon conjugation decreased from 18.9 nm for PluS NPs to 2.4 nm (for ZnP as an example) as determined by applying the Brunauer–Emmett–Teller method. The porphyrin complexes and their conjugates were tested for their photodynamic therapy (PDT) activity on MCF-7 breast cancer cells. It was found that ZnP and its conjugate showed the highest PDT activity. The p > 0.05 indicated that ZnP is significantly different than GaP and SiP.     

Synthesis,Optical and Photovoltaic Properties of Porphyrin Dyes

The synthesis and optical absorption of a series of porphyrins, and the photoelectrochemical properties of TiO₂ solar cells sensititized with these porphyrins was investigated. The different types of porphyrins studied are designated by numbers: the reference compound 1 (Zinc(II) 5,15-bis(4-carboxylphenyl)porphyrin), porphyrin substituted with one triarylamine unit 2, and porphyrin substituted with two triarylamine units 3. The UV-Vis absorption spectra reveal that the substitutions result in large redshifts in both the Soret band (～ 60 nm) and the Q bands (～ 125 nm), as well as enhancement of optical absorption. The enhancement is even more pronounced in the long-wavelength region of 575–725 nm, where the absorption of porphyrin 3 is eight times that of porphyrin 1. The photoelectrochemical properties of the porphyrins were also studied by constructing porphyrin-sensitized TiO₂ solar cells. Under standard AM 1.5 sunlight, the porphyrin 1 cell yields a short-circuit current of ～ 1.26 mA/cm², an open-circuit voltage of ～ 0.564 V, and a fill factor of ～ 61%. The incident photon-to-current conversion efficiency is ～ 24% for porphyrin 1 and ～ 5–7% for porphyrins 2 and 3 at the Soret peak.