以四磺基铝酞菁-牛血清白蛋白为底物的荧光恢复均相法测定胃蛋白酶

酸性介质中,红区荧光探针四磺基铝酞菁(AlS4Pc)的荧光被白蛋白显著猝灭,加入胃蛋白酶后,体系荧光明显回复。基于此现象,建立了荧光恢复均相测定胃蛋白酶的新方法。考察了各种影响因素,在最佳实验条件(pH2.5、反应温度50℃、反应时间1h)下,本方法的线性范围为0.04～4mg/L,检出限为20μg/L。用本方法测定实际样品中胃蛋白酶,取得了满意的结果。     

四磺基铝酞菁与爱尔新蓝的缔合作用在核酸定量中的应用

阴离子荧光染料四磺基铝酞菁与阳离子荧光染料爱尔新蓝的缔合作用 ,使四磺基铝酞菁发生荧光猝灭 ,而当核酸存在时 ,染料缔合平衡受到影响而导致四磺基铝酞菁的荧光恢复。根据这一原理 ,建立了核酸定量测定的新方法。方法具有很高的灵敏度和较好的选择性 ,其线性范围为 0～ 2 0 0 μg/L ;检测限分别为 1.8μg/L(SMDNA)、2 .0 μg/L(CTDNA)、5 .4μg/L(酵母RNA)。将方法用于实际样品金黄色葡萄球菌中DNA含量的测定 ,获得满意结果     

两亲性酞菁锌与牛血清白蛋白结合的研究

二磺基二邻苯二甲酰亚胺甲基酞菁锌(ZnPcS2P2)是一种具有卷动力活性的两亲性抗癌光敏剂，本文应用紫外吸收示差光谱、稳态和动态荧光光谱及平衡透析法研究了在生理条件下ZnPcS2P2与牛血清白蛋白(BSA)之间的相互作用。基于Hill位点模型，应用改进的蛋白内源荧光猝灭法求得ZnPcS2P2与BSA形成复合物的结合参数，结果与平衡透析法基本一致。     

甲磺基铝酞菁与爱尔新蓝的缔合作用在核酸定量中的应用

阴离子荧光染料四磺基铝酞菁与阳离子荧光染料爱尔新蓝的缔合作用，使四磺基铝酞菁发生荧光猝灭，而当核酸存在时，染料缔合平衡受到影响而导致四磺基铝酞菁的荧光恢复。根据这一原理，建立了核酸定量测定的新方法。方法具有很高的灵敏度和较好的选择性，其线性范围为0-200цg/L；检测限分别为1.8цg/L(SMDNA)、2.0цg/L(CTDNA)、5.4цg/L（酵母RNA）。将方法用于实际样品金黄色葡萄球菌中DNA含量的测定，获得满意结果。     

新型可溶性空心酞菁磺酰类化合物的合成及性质研究

以空心酞菁(H2Pc)为原料,采用取代基转化法,经过氯磺酰化和酯化合成了空心酞菁磺酰氯和空心酞菁磺酸对甲氧基苯酯,经元素分析,1H NMR,IR,UV-Vis等方法,确定了空心酞菁磺酰氯和空心酞菁磺酸对甲氧基苯酯的组成分别为H2Pc(SO2Cl)4和H2Pc(SO2-p-OC6H4OCH3)4.结果表明,此两种产物在空心酞菁的苯环上引入取代基后,长波吸收增强,溶解度高,热稳定性良好.     

含芘手性探针分子与蛋白质作用机理的时间分辨荧光光谱研究

采用时间分辨荧光光谱等手段研究了手性探针分子L-[4-(1-芘基)]丁酰基苯丙氨酸(PLP)与溶菌酶(Lys)、牛血清白蛋白(BSA)和人血清白蛋白(HSA)的结合过程及机理,探讨了三氯六氨合钴(CoHA)对不同复合体系内芘基的荧光猝灭作用.结果表明,PLP在与血清白蛋白的结合过程中是以芘基插入到血清白蛋白疏水空腔中的方式与蛋白质结合的;而PLP与Lys的结合部位处在其表面的疏水部分.     

喹诺酮药物与血清蛋白相互作用的三维荧光光谱研究

应用三维荧光光谱和三维荧光偏振光谱研究了数种喹诺酮药物与牛血清白蛋白(BSA)分子间的相互作用。由三维荧光(偏振)光谱得到的指纹信息说明了喹诺酮药物与BSA结合反应对BSA分子构象的影响。通过研究喹诺酮药物发生相互作用前后BSA荧光偏振度及各向异性的变化,定量说明了喹诺酮药物-BSA所发生的结合反应。     

对氯苯酚与牛血清白蛋白的相互作用研究

利用荧光光谱法研究了对氯苯酚(4-CP)与牛血清白蛋白(BSA)的相互作用,研究结果表明4-CP对BSA的荧光有较强的猝灭作用,其猝灭机理为静态猝灭,作用力主要为氢键和范德华力.依据Lineweaver-Burk方程和热力学方程获得了不同温度下水溶液和表面活性剂溶液中4-CP和BSA作用的结合常数、结合点位数及热力学参...     

四磺酸基酞菁锌的合成及其与牛血清白蛋白作用的研究

酞菁化合物及其金属配合物是一类光氧化还原反应的有效光敏剂,对恶性肿瘤具有荧光定位诊断和光动力治疗作用,并对金黄色葡萄球菌、链球菌以及某些寄生虫具有光灭活作用,已引起人们越来越多的兴趣[1].尤其是含不同数目磺酸取代基的酞菁金属配合物被认为是一种较有效的光动力治疗光敏剂.     

牛血清白蛋白与Indo-1相互作用的荧光光谱法研究

以牛血清白蛋白(Bovine serum albumin, BSA)与荧光探针Indo-1为蛋白质和配体模型, 基于Indo-1的荧光强度与BSA的分析浓度间的关系, 建立了计算二者相互作用位点数的方法, 并利用荧光共振能量转移及各种荧光技术对Indo-1和BSA的相互作用进行了研究. 结果表明, Indo-1在BSA中有3个作用位点, 这3个作用位点与BSA中的212位色氨酸(Trp 212)间的距离分别为2.93, 2.57和2.40 nm; Indo-1通过疏水性作用进入到BSA的3个疏水性空腔. 在荧光猝灭实验中, 通过Microlab 500 系列进样器和PTI荧光仪的联用实现了荧光强度的自动和实时记录.     

Time-gated fluorescence spectroscopy of porphyrin derivatives and aluminium phthalocyanine incorporated in vivo in a murine ascitic tumour model.

The effect of systemic administration on drug uptake at cellular level was evaluated using time-gated fluorescence spectroscopy performed on a murine ascitic tumour model. Mice bearing L1210 leukaemia were injected intraperitoneally or intravenously with 25 mg per kg body weight hematoporphyrin derivative (HpD), 12.5 mg per kg body weight photofrin II (PII), 25 or 5 mg per kg body weight disulphonated aluminium phthalocyanine (AlS2Pc). Every 2 h and for up to 22 or 30 h, mice were sacrificed, leukaemic cells extracted from the peritoneum, washed, and resuspended in buffer for fluorescence measurements. HpD and PII emission spectra were almost identical 12 h after intraperitoneal injection with main peaks at 630 nm and no appreciable changes afterwards. In the first 12 h, the PII fluorescence spectrum was constant, while in the case of HpD a shoulder at 615 nm was detectable. Similar fluorescence behaviour was observed after intravenous administration of porphyrin derivatives. These results seem to confirm that the tumour localizing fraction is the part actually retained by the cells. The AlS2Pc spectrum peaked at 685 nm and did not change in any of our experiments. AlS2Pc is incorporated more rapidly with respect to porphyrins, as was clearly observed in the case of intravenous administration, where the AlS2Pc fluorescence was readily detectable after 2 h, whereas the PII emission became apparent only after 4-6 h.     

Effects of photodynamic therapy on the absorption properties of disulphonated aluminum phthalocyanine in tumor-bearing mice

Time-resolved reflectance spectroscopy was performed on tumor-bearing mice, administered with disulphonated aluminum phthalocyanine (AlS(2)Pc, 5 mg/kg body weight), before, during and after photodynamic therapy. This allowed us to evaluate the absorption spectrum of AlS(2)Pc in vivo from 610 to 700 nm, and to investigate how the therapeutic irradiation affects it. Two tumor locations (intraderma on the back and intramuscular in the leg), and two uptake times (3 and 12 h) were considered. As already observed previously, the absorption spectrum of AlS(2)Pc in vivo is centered at 680-685 nm. The irradiation causes a blue-shift of the measured line shape, more or less marked depending on the experimental conditions. A reduction in absorption is also often observed upon illumination with therapeutic light doses.     

Direct near-infrared luminescence detection of singlet oxygen generated by photodynamic therapy in cells in vitro and tissues in vivo

Singlet oxygen (1O2) is believed to be the major cytotoxic agent involved in photodynamic therapy (PDT). Measurement of 1O2 near-infrared (NIR) luminescence at 1270 nm in biological environments is confounded by the strongly reduced 1O2 lifetime and probably has never been achieved. We present evidence that this is now possible, using a new NIR-sensitive photomultiplier tube. Time-resolved 1O2 luminescence measurements were made in various solutions of aluminum tetrasulphonated phthalocyanine (AlS4Pc) and Photofrin. Measurements were also performed on suspensions of leukemia cells incubated with AlS4Pc, and a true intracellular component of the 1O2 signal was clearly identified. Time-resolved analysis showed a strongly reduced 1O2 lifetime and an increased photosensitizer triplet-state lifetime in the intracellular component. In vivo measurements were performed on normal skin and liver of Wistar rats sensitized with 50 mg/kg AlS4Pc. In each case, a small but statistically significant spectral peak was observed at 1270 nm. The 1O2 lifetime based on photon count rate measurements at 1270 nm was 0.03-0.18 micros, consistent with published upper limits. We believe that these are the first direct observations of PDT-generated intracellular and in vivo 102. The detector technology provides a new tool for PDT research and possibly clinical use.     

Fluorescence imaging during photodynamic therapy of experimental tumors in mice sensitized with disulfonated aluminum phthalocyanine

A fluorescence imaging system was used to monitor the emission of disulfonated aluminum phthalocyanine (AlS2Pc) during the photodynamic therapy (PDT) of murine tumors. Cells of the MS-2 fibrosarcoma were injected in mice in two compartments in order to cause the development of tumors in different host tissues. Two drug doses and two uptake times were considered. Moreover, the fluorescence of the AlS2Pc was excited using two wavelengths on the opposite sides of the absorption peak to detect a possible change in the absorption spectrum of the sensitizer induced by the PDT. In the tumors, the treatment induces a variation of the fluorescence intensity: in some mice a mild photobleaching takes place, in others a fluorescence enhancement occurs. Which effect predominates depends on the experimental conditions, even though a large spread of data was found amongst mice of the same group. In all mice, independently of the drug dose, uptake time or tumor compartment, a marked increase in the fluorescence signal takes place at the borders of the irradiated area. To quantify this effect we evaluated the ratio between the fluorescence intensities in the peritumoral area and in the tumor itself. This ratio increases monotonically during the PDT, showing a different behavior with the two excitation wavelengths. This indicates that the AlS2Pc absorption spectrum shifts toward shorter wavelengths as a result of the irradiation.     

N-烷基-N,N-二(2-羟乙基)-N-甲基溴化铵与牛血清白蛋白的相互作用

用荧光光谱法在298K研究了Tris-HCl缓冲溶液(pH=7.1)中系列N-烷基-N,N-二(2-羟乙基)-N-甲基溴化铵(烷基链长为C12到C16)与牛血清白蛋白(BSA)的结合作用,考察了表面活性剂结构、BSA浓度对结合作用的影响,分别用Stern-Volmer方程、虚拟结合常数模型探讨了表面活性剂在浓度较低区域与BSA的作用机制.结果表明:三种季铵盐表面活性剂均对BSA内源荧光有猝灭作用,并导致其最大发射波长蓝移;表面活性剂的烷基链越长,Stern-Volmer猝灭常数和虚拟结合常数越大,表面活性剂与BSA的结合作用也越强.     

Determination of proteins with tetracarboxy manganese(II) phthalocyanine by resonance light scattering technique

A novel method for the determination of proteins by using tetracarboxy manganese(II) phthalocyanine (MnC4Pc) as a resonance light scattering (RLS) probe has been developed. At pH 3.0 Britton-Robinson (B-R) buffer solution, the RLS intensity of MnC4Pc at 385 nm is greatly enhanced in the presence of proteins. The effects of pH, reaction time, concentration of MnC4Pc and interfering substances on the enhanced RLS intensity are investigated, respectively. Under optimal conditions, the linear ranges of the calibration curves are 0-2.00 microg mL(-1) for bovine serum albumin (BSA) and human serum albumin (HSA), 0.0-1.75 microg mL(-1) for human-IgG and ovalbumin, with a detection limit of 16.37 ng mL(-1) BSA, 17.62 ng mL(-1) HSA, 19.41 ng mL(-1) human-IgG and 20.72 ng mL(-1) ovalbumin. The method has been applied to the determination of total proteins in human serum samples collected from a hospital and the results are in good agreement with those reported by the hospital.     

Preparation of (2E)-3-(4'-Halophenyl)prop-2-enoyl Sulfachlorpyridazine Sodium Salts and Their Interaction with Bovine Serum Albumin by Fluorescence Spectroscopy

Three (2E)-3-(4'-halophenyl)prop-2-enoyl sulfachlorpyridazine sodium salts(XPSCA) were synthesized. Their chemical structures were confirmed by ¹H NMR and ¹³C NMR, electrospray ionization mass spectrometry (ESI-MS), and infrared(IR) spectroscopy. The interactions between XPSCA and bovine serum albumin(BSA) were investigated under imitated physiological condition by fluorescence quenching technique and UV-Vis absorption spectroscopy according to the Stern-Volmer equation. The results from the emission quenching at different temperatures indicate that the quenching mechanism of serum albumin by XPSCA was static quenching mechanism at low XPSCA concentrations or a combined quenching(static and dynamic) mechanism at higher XPSCA concentrations. At different temperatures, the binding constant and the binding sites of XPSCA with BSA were investigated, and the distances were evaluated according to Förster non-radiative resonance energy transfer theory. The thermodynamic parameters were calculated according to van't Hoff equation, which implies that both van der Waals interaction and hydrogen bond played major roles in stabilizing the XPSCA-BSA complexes, whereas hydrophobic interactions were secondary. Moreover, the conformational changes in BSA were analyzed by synchronous fluorescence spectra.     

含喹唑啉酮的4-(4-氟苯基)哌嗪二硫代甲酸酯与牛血清白蛋白相互作用的荧光光谱研究

用荧光光谱法研究了具有抑制人肿瘤细胞活性的含喹唑啉酮的4-(4-氟苯基)哌嗪二硫代甲酸酯与牛血清白蛋白的相互作用。结果表明:在生理条件下,它对牛血清白蛋白的荧光有较强的猝灭作用。根据猝灭结果,求得了不同温度下反应的结合位点数、结合常数及反应热力学参数,并据此确定了它们相互作用的主要形式。     

Studies of (3-mercaptopropyl)trimethoxylsilane and bis(trimethoxysilyl)ethane sol–gel coating on copper and aluminum

Berbamine, a naturally occurring isoquinoline alkaloid extracted from Berberis sp., is the active constituent of some Chinese herbal medicines and exhibits a variety of pharmacological activities. The effects of berbamine on the structure of bovine serum albumin (BSA) were investigated by circular dichroism, fluorescence and absorption spectroscopy under physiological conditions. Berbamine caused a static quenching of the intrinsic fluorescence of BSA, and the quenching data were analyzed by application of the Stern–Volmer equation. There was a single primary berbamine-binding site on BSA with a binding constant of 2.577 × 10⁴ L mol⁻¹ at 298 K. The thermodynamic parameters, enthalpy change (ΔH⁰) and entropy change (ΔS⁰) for the reaction were −76.5 kJ mol⁻¹ and −173.4 J mol⁻¹ K⁻¹ according to the van’t Hoff equation. The results showed that the hydrogen bond and van der Waals interaction were the predominant forces in the binding process. Competitive experiments revealed a displacement of warfarin by berbamine, indicating that the binding site was located at Drug sites I. The distance r between the donor (BSA) and the acceptor (berbamine) was obtained according to the Förster non-radiation energy transfer theory. The results of three-dimensional fluorescence spectra, UV–vis absorption difference spectra and circular dichroism of BSA in the presence of berbamine showed that the conformation of BSA was changed. The results provide a quantitative understanding of the effect of berbamine on the structure of bovine serum albumin, providing a useful guideline for further drug design.     

Study of the interaction between 2,5-di-[2-(4-hydroxy-phenyl)ethylene]-terephthalonitril and bovine serum albumin by fluorescence spectroscopy

A new compound, 2,5-di-[2-(4-hydroxy-phenyl)ethylene]-terephthalonitrile (DHPEPN), was synthesized. The interaction between bovine serum albumin (BSA) and DHPEPN in Tris-HCl buffer solution (pH 7.4) was investigated using fluorescence and UV-vis absorption spectroscopy. The mechanism of BSA fluorescence quenched by DHPEPN is discussed according to the Stern-Volmer equation. The binding constant and the thermodynamic parameters ΔH, ΔS, ΔG at different temperatures were calculated. The results indicate that the van der Waals interaction and hydrogen bonding play major roles in the binding process. The distance between BSA and DHPEPN is estimated to be 3.59 nm based on the F?rster resonance energy transfer theory. The spectral changes of synchronous fluorescence and three-dimensional fluorescence suggest that both of the microenvironment of DHPEPN and the conformation of BSA are changed during binding between DHPEPN and BSA.