Photochemical reaction of magnesium tetraphenyl porphyrin with sulfur dioxide

<正>The photochemical reaction of magnesium tetraphenyl porphyrin(MgTPP) with sulfur dioxide(SO_2) was investigated in dichloromethane(CH_2Cl_2) by steady-state fluorescence,UV-vis absorption,MS,and XRD spectroscopic techniques.These spectra showed that under irradiation MgTPP reacted with SO_2 to form 1:1 molecular adduct at first step.During the process of keeping irradiation and maintaining the flow of SO_2,SO_2 was reduced into S~(2-) by MgTPP and the results were detected using MS and XRD techniques.Understanding the photochemical reaction of MgTPP with SO_2 is of key interest in elucidating fundamental photochemical reaction mechanisms associated with this class of chlorophyll in the presence of SO_2.     

Photochemical fixation and reduction of sulfur dioxide to sulfide by tetraphenylporphyrin magnesium: Spectroscopic and kinetic studies

The photochemical reaction of sulfur dioxide(SO2) with tetraphenylporphyrin magnesium(MgTPP) has been investigated in dichloromethane(CH2Cl2) solution at room temperature with illumination by visible light.Conventional fluorescence,UV-vis,and MS spectral analyses showed that under these conditions,SO2 was initially photochemically fixed by MgTPP to form a 1:1 molecular adduct.On continued irradiation and maintaining the flow of SO2,MS and XRD results showed that MgTPP is remarkably effective in the photochemical reduction of SO2 to sulfide(S2).The kinetics of the photochemical reaction of MgTPP with SO2 was studied in a SO2-saturated solution.Under irradiation,the reaction follows pseudo first order kinetics for MgTPP,having a half-life decreasing from 106 to 57 min as the illumination intensity is increased from 350 to 600 Lm.This investigation of the photochemical fixation and reduction of SO2 by MgTPP is of key interest in elucidating fundamental photochemical reaction mechanisms associated with porphyrins in the presence of SO2 ;furthermore,the analysis of the photochemical reaction may offer new opportunities for the fixation and reduction of SO2 to less harmful species.     

Spectral studies of the interaction between sanguinarine and guanosine

The interaction between sanguinarine and guanosine was investigated by using UV-vis and fluorescence spectra at pH 7.2. The binding of sanguinarine to guanosine was substantiated by the hypochromism and bathochromism in the absorption spectra and the emission quenching in fluorescence spectra. The fluorescence lifetime results, the varieties of the fluorophore absorption spectra and the decrease of the binding constant with the increasing temperature all indicate that the fluorescence quenching is static. The ratio and constant of the binding cytidine to sanguinarine are 2 and 6.44 × 10^7, respectively. The result shows that the binding of sanguinarine to guanosine is not only exothermic but also entropy-driven with △H=-8.53kJ/mol, AS = 0.12 kJ/（molK）, and AG =-44.57 kJ/mol at 298.15 K.     

Photochemical reaction between magnesium tetraphenyl porphyrin and oxygen

The photochemical reaction of magnesium tetraphenyl porphyrin （MgTPP） with O2 was studied in CH2Cl2 by steady-state fluorescence, UV-vis absorption, FTIR and MALDI-TOF MS measurements. These spectra indicate that O2 can react with MgTPP excited by irradiation, forming the stable 1：1 coordinated adduct of MgTPP-O2. In the adduct, the oxygen atoms of O2 may insert in the Mg-N bonds in MgTPP and bind with the nitrogen atoms of MgTPP to form N-O-Mg bonds.     

钴卟啉对三种胺的固定用于SO2的脱除

利用紫外-可见光谱和荧光光谱手段研究了四苯基卟啉钴（CoTPP）对苯胺、乙二胺和二乙胺的超分子固定用于脱除SO2. 紫外-可见光谱表明CoTPP与三种胺作用后生成CoTPP-胺配合物,Soret吸收带发生红移. 当通入SO2后,SO2与胺的作用强于CoTPP与胺的作用,CoTPP-胺配合物释放出CoTPP,CoTPP 在胺法脱硫过程中起到胺固定作用. 荧光光谱表明CoTPP与三种胺作用形成1：1的分子配合物,且为熵驱动反应. CoTPP与苯胺和二乙胺作用为吸热反应,CoTPP与乙二胺作用为放热反应.     

磁性纳米氧化铁与CdTe量子点相互作用的光谱学研究

采用荧光光谱及紫外-可见吸收光谱研究了不同条件下磁性纳米氧化铁(MION)与CdTe量子点的相互作用, 发现MION对CdTe量子点荧光有猝灭作用. 由Stern-Volmer方程分析得到MION与CdTe量子点结合反应的荧光猝灭速率常数K_q值为7.68×10¹⁵ mol•L^－1•s^－1, 结合紫外-可见吸收光谱进一步证实此过程为静态猝灭过程. 并由Lineweaver-Burk方程得到MION与CdTe量子点结合的热力学焓变(?H^?)值为21.6 kJ•mol^－1、熵变(?S^?)值为210.3 J• mol^－1•K^－1和自由能变(?G^?)值为－41.1 kJ•mol^－1 (298 K). 对其相互作用机理进行探讨, 结果表明MION对CdTe量子点作用为自发过程, 主要存在静电作用.     

Facile synthesis of N-acetyl-L-cysteine capped ZnS quantum dots as an eco-friendly fluorescence sensor for Hg2+

This paper described an investigation of a novel eco-friendly fluorescence sensor for Hg²⁺ ions based on N-acetyl-l-cysteine (NAC)-capped ZnS quantum dots (QDs) in aqueous solution. By using safe and low-cost materials, ZnS QDs modified by NAC were easily synthesized in aqueous medium via a one-step method. The quantitative detection of Hg²⁺ ions was developed based on fluorescence quenching of ZnS QDs with high sensitivity and selectivity. Under optimal conditions, its response was linearly proportional to the concentration of Hg²⁺ ions in a range from 0 to 2.4 × 10⁻⁶ mol L⁻¹ with a detection limit of 5.0 × 10⁻⁹ mol L⁻¹. Most of common physiologically relevant cations and anions did not interfere with the detection of Hg²⁺. The proposed method was applied to the trace determination of Hg²⁺ ions in water samples. The possible quenching mechanism was also examined by fluorescence and UV-vis absorption spectra.     

Synchronous fluorescence determination of DNA based on the interaction between methylene blue and DNA

The fluorescence intensity of methylene blue (MB) quenched by DNA in the pH range of 6.5-8.0 was studied with synchronous fluorescence technology. A novel method for detecting single-stranded and double-stranded DNA was developed. The decreased fluorescence intensity at 664 nm is in proportion to the concentration of DNA in the range of 0.28-11.0 μmol L⁻¹ for ctDNA, 0.14-8.25 μmol L⁻¹ for thermally denatured ctDNA and 0.28-8.25 μmol L⁻¹ for hsDNA. The detection limits (S/N = 3) are 0.11, 0.04 and 0.04 μmol L⁻¹, respectively. The method is rapid, selective, and the reagents are lower toxic. It has been used for the determination of DNA in synthetic samples with good satisfaction. In addition, the interaction modes between MB and ctDNA and the mechanism of the fluorescence quenching were also discussed in detail. The experimental results from absorption spectra and fluorescence polarization indicate that the possible interaction modes between MB and DNA are the electrostatic binding and the intercalation binding.     

Cr（VI）与牛血清白蛋白的相互作用

采用荧光光谱、紫外光谱、CD光谱法研究了K2Cr2O7与牛血清白蛋白(BSA)的相互作用。实验结果表明, 铬(Ⅵ)使BSA的紫外吸收降低,峰位红移,表明铬(Ⅵ)与BSA发生较强的相互作用;铬(Ⅵ)酸根离子与BSA形成基态复合物导致BSA内源荧光猝灭,猝灭机理主要为静态猝灭。测定了不同温度下该反应的热力学参数,ΔGθ＜0,ΔHθ和ΔSθ分别为–12.60 kJ/mol 和 56.60 J/(mol·k), 表明上述作用过程是一个熵增加、自由能降低的自发分子间作用过程,铬(Ⅵ)酸根离子与BSA之间以静电作用力为主;非辐射能量转移机理确定了铬(Ⅵ)与牛血清白蛋白中色氨酸残基之间的距离 r＝2.85 nm;同步荧光和CD光谱研究表明,铬(Ⅵ)使BSA的二级结构发生改变,α–螺旋含量降低,色氨酸残基所处微环境的极性减小。     

Synthesis and characterization of polyaniline nanoparticles in the presence of magnetic field and samarium chloride

A new and economical method of preparing polyaniline (PANI) nanoparticles will be introduced in this article. Compared with conventional methods, this method is much more simple and convenient. Scanning electron microscope (SEM) shows that the diameter of particles are between 30 and 50 nm, which is in good agreement with the results of a transmission electron microscope (TEM). Polyaniline/SmCl₃/Bp, polyaniline/SmCl₃ and polyaniline/HCl were prepared in a solution containing 1.0 mol dm⁻³ aniline, 1.0 mol dm⁻³ HCl with and without 0.5 mol dm⁻³ SmCl₃, in the presence and in the absence of a magnetic field, respectively. Their conductivity, UV-vis spectra, FTIR spectra, X-ray diffraction (XRD) and thermogravimetric analysis (TGA) were investigated. Changes in UV-vis and FTIR spectra indicate a strong interaction between Samarium ions (SmCl₃) and polyaniline chains. The conductivity of PANI depends on magnetization and concentration of Sm³⁺. Polyaniline/SmCl₃/Bp has the higher degree of crystallinity than that of polyaniline/HCl.     

Chelerythrine chloride binding of guanosine in aqueous solution

In this work, the interaction between chelerythrine (CHE) and guanosine is studied using UV-vis and fluorescence measurements at various temperatures. The UV-vis spectra show that the increasing guanosine concentrations result in the decreasing absorption intensity and red shift of CHE E absorption band (267 nm). The fluorescence spectra are fitted to linear analysis, yielding a binding constant of 1.04×104 L/mol at 298.15 K of CHE with guanosine. Besides, with △rHΘm =-8.26 kJ/mol, △rGmΘ = -22.90 kJ/mol,and △rSmΘ = 49.38 J/(mol K) the interaction should be entropy-driven and exterothermic.     

Stoichiometries and thermodynamic stabilities for aqueous sulfate complexes of U(VI)

The formation constants of UO2SO4 (aq), UO2(SO4)2(2-), and UO2(SO4)3(4-) were measured in aqueous solutions from 10 to 75 degrees C by time-resolved laser-induced fluorescence spectroscopy (TRLFS). A constant enthalpy of reaction approach was satisfactorily used to fit the thermodynamic parameters of stepwise complex formation reactions in a 0.1 M Na(+) ionic medium: log 10 K 1(25 degrees C) = 2.45 +/- 0.05, Delta r H1 = 29.1 +/- 4.0 kJ x mol(-1), log10 K2(25 degrees C) = 1.03 +/- 0.04, and Delta r H2 = 16.6 +/- 4.5 kJ x mol(-1). While the enthalpy of the UO2(SO4)2(2-) formation reaction is in good agreement with calorimetric data, that for UO2SO4 (aq) is higher than other values by a few kilojoules per mole. Incomplete knowledge of the speciation may have led to an underestimation of Delta r H1 in previous calorimetric studies. In fact, one of the published calorimetric determinations of Delta r H1 is here supported by the TRLFS results only when reinterpreted with a more correct equilibrium constant value, which shifts the fitted Delta r H1 value up by 9 kJ x mol(-1). UO2(SO 4) 3 (4-) was evidenced in a 3 M Na (+) ionic medium: log10 K3(25 degrees C) = 0.76 +/- 0.20 and Delta r H3 = 11 +/- 8 kJ x mol(-1) were obtained. The fluorescence features of the sulfate complexes were observed to depend on the ionic conditions. Changes in the coordination mode (mono- and bidentate) of the sulfate ligands may explain these observations, in line with recent structural data.     

Synthesis, spectrophotometric pH titrations and DNA binding properties of a cyclometalated iridium(III) complex of tetrapyrido[3,2-a:2′,3′-c:3″,2″-h:2?,3?-j]phenazine

A new cyclometalated iridium(III) complex [Ir(ppy)₂(tpphz)]Cl {Hppy = 2-phenylpyridine and tpphz = tetrapyrido[3,2-a:2′,3′-c:3″,2″-h:2?,3?-j]phenazine} has been synthesized and characterized. The pH effects on UV-vis absorption spectra have been studied, and three ground-state acidity ionization constant values have been derived. The calf thymus (ct) DNA binding properties of the complex have also been investigated with UV-vis absorption spectrophotometric titrations, DNA competitive binding with ethidium bromide, DNA melting experiments, viscosity measurements, and density functional theory calculations. The complex was demonstrated to act as a DNA intercalator with a binding constant of (9.29 ± 1.26) × 10⁵ M⁻¹ more than one order of magnitude greater than that previously reported for DNA intercalator of [Ir(ppy)₂(dppz)]⁺.     

四苯基卟啉镁的合成、表征及光化学性质

提出一种以乙酸镁和乙酸钠为原料合成四苯基卟啉镁(MgTPP)的新方法, 合成样品以柱层析法进行分离纯化. 分离产物经UV-Vis、1H-NMR、MALDI-TOF-MS(基质辅助激光解吸电离飞行时间质谱)等技术表征, 确定为MgTPP. UV-Vis光谱分析结果表明, 四苯基卟啉镁的Soret 吸收带为424 nm, Q 吸收带为563 nm 和602 nm. 此外, 光照对MgTPP的二氯甲烷溶液光谱性质的影响结果表明, 经光照射后MgTPP的UV-Vis光谱的Soret吸收带吸收强度明显降低, 同时, 经550 nm的光激发产生的荧光有明显的猝灭. 对光照后的MgTPP样品进行MALDI-TOF-MS分析, 发现有新的质核比(m/z)出现, 其为668, 这一结果表明, 在光照条件下, MgTPP分子可能与氧分子发生光化学作用, 形成MgTPP与氧的复合物MgTPP-O2.     

Mechanism and conformational studies of farrerol binding to bovine serum albumin by spectroscopic methods

The mechanism and conformational changes of farrerol binding to bovine serum albumin (BSA) were studied by spectroscopic methods including fluorescence quenching technique, UV–vis absorption, circular dichroism (CD) spectroscopy and Fourier transform infrared (FT-IR) spectroscopy under simulative physiological conditions. The results of fluorescence titration revealed that farrerol could strongly quench the intrinsic fluorescence of BSA through a static quenching procedure. The thermodynamic parameters enthalpy change and entropy change for the binding were calculated to be −29.92 kJ mol⁻¹ and 5.06 J mol⁻¹ K⁻¹ according to the van’t Hoff equation, which suggested that the both hydrophobic interactions and hydrogen bonds play major role in the binding of farrerol to BSA. The binding distance r deduced from the efficiency of energy transfer was 3.11 nm for farrerol–BSA system. The displacement experiments of site markers and the results of fluorescence anisotropy showed that warfarin and farrerol shared a common binding site I corresponding to the subdomain IIA of BSA. Furthermore, the studies of synchronous fluorescence, CD and FT-IR spectroscopy showed that the binding of farrerol to BSA induced conformational changes in BSA.     

Reactions of cis-(aqua)(amine)bis(ethylenediamine)cobalt(III) complexes with sulfur(IV) in aqueous medium

The kinetics of the formation/acid-catalysed aquation (SO2 elimination), CoIII-OSO2+CoIII-SO3+ isomerization, intramolecular reduction and base hydrolysis of the O-bonded sulfito complexes, cis-[Co(en)2(RNH2) (OSO2)]+ (en=ethylenediamine; R=H, Me, Et, PhCH2 and C6H11) have been investigated. The spontaneous and base-catalysed isomerization involve loss of monodentate amine ligands from the CoIII centre to give trans-[Co(en)2(SO3-S)2]– (in excess SO32–) or trans-[Co(en)2(OH)(SO3-S)] (under base hydrolysis conditions). This result is presumably associated with a cis-labilizing action of the O-bonded sulfite. Steric retardation is observed for the formation and acid-catalysed aquation of the O-sulfito complex, the effect being relatively larger for the latter reaction. Steric acceleration is observed in the isomerization and intramolecular reduction and base hydrolysis of the O-sulfito complexes.¶ The trans-S-disulfito complex is prone to fast H+-catalysed aquation {k=(1.52±0.06)×104 dm3 mol–1 s–1, H=81 ± 2 kJ mol–1, S= 108 ± 5 J K–1 mol–1 at 25°C, I = 1.0 mol dm–3} yielding trans-[Co(en)2 (SO3-S)(OH2)]+.     

Dual responsive chemosensors for anions: the combination of fluorescent PET (Photoinduced Electron Transfer) and colorimetric chemosensors in a single molecule

The design and synthesis of two novel fluorescent PET anion sensors is described, based on the principle of ‘fluorophore-spacer-(anion)receptor’. The sensors 1 and 2 employ simple diaromatic thioureas as anion receptors, and the fluorophore is a naphthalimide moiety that absorbs in the visible part of the spectrum and emits in the green. Upon recognition of anions such as F⁻ and AcO⁻ in DMSO, the fluorescence emission of 1 and 2 was ‘switched off’, with no significant changes in the UV-vis spectra. This recognition shows a 1:1 binding between the receptor and the anions. In the case of F⁻, further additions of the anion, gave rise to large changes in the UV-vis spectra, where the λ_max at 455 nm was shifted to 550 nm. These changes are thought to be due to the deprotonation of the 4-amino moiety of the naphthalimide fluorophore. This was in fact found to be the case, using simple naphthalimide derivatives such as 6. Sensors 1 and 2 can thus display dual sensing action; where at low concentrations, the fluorescence emission is quenched, and at higher concentrations the absorption spectra are modulated.     

Interaction between quercetin-copper(II) complex and DNA with the use of the Neutral Red dye fluorophor probe

The interaction of quercetin-Cu(II) complex with calf thymus DNA was investigated with the use of Neutral Red (NR) dye as a spectral probe by the application of UV-vis spectrophotometry, cyclic voltammetry and synchronous fluorescence spectroscopy. The results showed that both quercetin-Cu(II) complex and the NR molecule can intercalate into the double helix of the DNA. The 2:1 quercetin:Cu(II) complex (estimated binding constant = 2.85 × 10⁹) is stabilized by intercalation in the DNA (binding constant, K_{[quercetin-Cu(II)-DNA]} = (1.82 ± 0.20) × 10⁵ M⁻¹), and displaces the NR dye from the NR-DNA complex in a competitive reaction. Cyclic voltammetry studies confirm the intercalation reaction and show that the ratio (K_R/K_O) of binding constants for the reduced and oxidized forms of the metal complex is 2.05. Furthermore, the alternative least squares (ALS) method was applied to resolve a complex two-way array of the absorption spectra data. This yielded the equilibrium concentration profiles of each component in the reaction (NR, NR-DNA and quercetin-Cu(II)) as well as the corresponding pure spectra. The extracted profiles showed that at equilibrium the [NR-DNA] and [NR] trends decreased and increased symmetrically, respectively, with approximately linear behaviour being observed below 10 × 10⁻⁶ mol L⁻¹ of the added quercetin-Cu²⁺ complex. Thereafter, these trends converged asymptotically. The free [quercetin-Cu(II)] trend-line at equilibrium was linear over the whole range of the complex added. It was possible to estimate the approximate value of the equilibrium constant of the exchange process (approximately 5 × 10⁻¹) involving the intercalation of the quercetin-Cu(II) complex. It was also found that about 35% of the bound complex was unaccounted by the intercalation reaction, presumably being stabilized at an alternative site.     

Comparison of synchronous and laser-induced fluorescence spectroscopy applied to the Eu(III)-fulvate complexation

The complexation of europium ion (Eu(III)) with a soil fulvic acid (FA) has been studied at pH 5 in 0.01 M NaClO₄ by different experimental methods, i.e. synchronous fluorescence spectroscopy (SyFS) and time resolved laser-induced fluorescence spectroscopy (TRLFS). A series of SyFS quenching spectra was obtained by increasing the Eu(III) concentration and keeping the FA concentration constant. The emission spectra and fluorescence lifetimes of the Eu(III) bound to the FA were also measured by a TRLFS system using the same solution used in the SyFS spectral measurement. From the analysis of the fluorescence data obtained by the SyFS and the TRLFS using a non-linear least-squares method, the concentration of the binding sites (C_L) of the FA accessible for the Eu(III) and the corresponding conditional stability constants (log K) were estimated. The two different methods gave rise to constants being comparable with one another. The log K and C_L values (mean ± standard deviation of three determinations) determined by the SyFS were 6.4 ± 0.2 (6.7 ± 0.1 μmol L⁻¹: by the TRLFS) and 10 ± 1 μmol L⁻¹ (7 ± 1 μmol L⁻¹: by the TRLFS), respectively. The applicability of the FA fluorescence quenching techniques for estimating the europium binding parameters was proved by the direct monitoring of the Eu(III) bound to the FA using the TRLFS system.     

Chlorobenzylidine-herring sperm DNA interaction: binding mode and thermodynamic studies

The interaction of chlorobenzylidine with herring sperm DNA has been investigated by fluorescence, absorption, DNA melting experiment and differential scanning calorimetry (DSC). When bound to DNA, chlorobenzylidine shows hypochromism and red shift in absorption spectra, fluorescence quenching and polarization increasing in fluorescence spectra and increasing in DNA melting temperature. These spectral characteristics strongly support intercalation of chlorobenzylidine into herring sperm DNA. Scatchard plots constructed from fluorescence titration data give a binding constant of 3.2 x 10(4) M(-1) and a binding site size of six base pairs per bound drug molecule. The intercalative interaction is exothermic with a van't Hoff enthalpy of -30.6 kJ mol(-1). This result is obtained from DSC experiment. In addition, DeltaG degrees =-28.5 kJ mol(-1), and DeltaS degrees =-7.1 J mol(-1) K(-1). These results show that the binding of chlorobenzylidine to herring sperm DNA is exothermic.