OPTICAL EXCITATION OF THE EOSIN-HUMAN SERUM ALBUMIN COMPLEX*

Abstract The excitation of the eosin-human serum albumin complex has been investigated with spectral and photochemical techniques. Measurements of the changes in absorption and fluorescence spectra induced by complexing have shown that the first eosin molecule is held more strongly than the next few and that multiple binding leads to an enhanced fluorescence self-quenching. Flash photolytic measurements indicate that dye-dye quenching interactions enhance triplet eosin formation, and that oxygen quenching of the triplet is suppressed when the dye is singly bound. The quantum yield for aerobic photobleaching of the complex has been measured and is interpreted in terms of these findings.     

头孢拉定与血清白蛋白相互作用的光谱学研究

采用荧光和紫外吸收光谱法研究头孢拉定和牛血清白蛋白(BSA)的相互作用.研究发现,头孢柱定荧光猝灭牛血清白蛋白是由于形成了头孢拉定-牛血清白蛋白复合物.分别计算了不同温度下双分子猝灭常数kq和结合常数K.由热力学参数焓变(△H)、熵变(△S)和吉布斯自由能(△G),推断出头孢拉定与BSA的相互作用是一个疏水作用的自发过...     

HEMATOPORPHYRIN PHOTOSENSITIZATION OF SERUM ALBUMIN and SUBTILISIN BPN'

—The photosensitized inactivation of subtilisin BPN' by free hematoporphyrin (HP) followed exponential kinetics with positive mechanistic tests for the involvement of singlet oxygen (¹O₂) as the principal intermediate. The photoinactivation quantum yield was 0.029 at 390 nm in oxygen-saturated, D₂O buffer at pH 7.0. The effects of HP binding were investigated for tryptophan oxidation in bovine serum albumin (BSA) and human serum albumin (HSA) at high protein:HP concentration ratios where the HP was > 97% complexed. The reaction kinetics were non-exponential and mimick a second-order process in the initial stages. The rate of HP photobleaching was 30-fold faster for complexed HP compared with free HP, which was shown to account for the observed kinetics. Mechanistic tests showed that ¹O₂ was the dominant photooxidizing intermediate of tryptophan residues and that it was not involved in the accompanying photobleaching of HP. The quantum yield for tryptophan oxidation in BSA was 0.11 at 390 nm in oxygen-saturated, D₂O buffer at pH 8.0. The reactivity of HSA was approximately 2-fold lower than BSA for equivalent conditions. Estimates of the reaction cross sections led to 3 Ų for the inactivation of subtilisin BPN' by ¹O₂ and 20 Ų for the oxidation of tryptophan in BSA.     

荧光光谱法研究美托拉宗与牛血清白蛋白的相互作用

采用荧光光谱技术研究了在pH7.40的Tris-HCl缓冲介质中美托拉宗与BSA相互作用。实验发现,美托拉宗对BSA有较强的荧光猝灭作用,根据292K和311K时美托拉宗对BSA的荧光猝灭作用,利用Stern-Volmer方程及双倒数方程处理实验数据,表明美托拉宗对BSA的荧光猝灭作用属于动态猝灭过程,根据F rster非辐射能量转移理论计算出了美托拉宗与BSA间的结合距离r=2.77 nm,结合过程的热力学数据表明,二者主要靠疏水作用力结合;进一步采用同步荧光光谱探讨了美托拉宗对BSA构象的影响。     

荧光光谱法研究橙皮甙与牛血清白蛋白的相互作用

在pH7.40的Tris-HCl 缓冲体系中,采用荧光光谱技术研究了橙皮甙与牛血清白蛋白(BSA)的相互作用.随着温度升高,橙皮甙与BSA 的猝灭常数逐渐增加.实验表明:橙皮甙对BSA的荧光猝灭为动态猝灭过程.由热力学参数焓变(△H=70.71 kJ/mol)大于零和熵变[△S=316.29J/(mol·K)]大于零,...     

光谱法研究绿原酸与人血清白蛋白的相互作用

利用荧光光谱法研究了绿原酸与人血清白蛋白(HSA)的相互作用,考察了不同温度下绿原酸与HSA的结合常数KA和结合位点数n,并研究了Cu2+、Al3+、Ca2+、Pb2+等金属离子对绿原酸与HSA结合性质的影响。基于Frster偶极-偶极非辐射能量转移机理确定了荧光给体HSA与受体绿原酸间的结合距离。     

SPECTRAL STUDY OF THE PHOTOCHEMISTRY OF DIPYRROLE MODELS FOR BILIRUBIN BOUND TO HUMAN SERUM ALBUMIN

—Dipyrromethenones, which include xanthobilirubinic acid (I), its methyl ester (II) and the endo- vinyl analog of neoxanthobilirubinic acid methyl ester ("half bilirubin" methyl ester) (III) bind to human serum albumin (HSA) and thereby exhibit greatly increased fluorescence as well as induced circular dichroism in their long wavelength transitions. As determined from fluorescence studies, the "tightness" of the binding to HSA is, inter alia , inversely related to the inherent solubility of the dipyrromethenone in aqueous buffer. Fast (ps) configurational isomerization ( Z → E ) is the major pathway for decay of the first excited (singlet) states of the HSA-bound dipyrromethenones. A quantum yield of − 0.4 is associated with the Z → E isomerization. Binding to HSA enhances the lifetimes of the less thermodynamically stable E -isomers. The results of these studies of "half bilirubins" allow a clear evaluation of the effects of protein binding upon the photophysics and photochemistry of bilirubin.     

PHOTOCHEMISTRY OF MODIFIED PROTEINS BENZOPHENONE-CONTAINING BOVINE SERUM ALBUMIN

Abstract— The results of exploratory and mechanistic studies of the photochemistry of poly- p -benzoyl-acetimido-bovine serum albumin, a modified protein containing photoreactive and photosensitizing groups, are reported. Specifically described are our recent findings concerning (1) the synthesis and characterization of a modified bovine serum albumin that contains benzophenone-like moieties, (2) the photochemistry of this modified protein which appears to involve photoreductive coupling of the benzophenone chromophores to the protein backbone, and (3) triplet energy transfer from modified bovine serum albumin to small molecule acceptors resulting in quenching of the photoreaction.     

BINDING OF HEMATOPORPHYRIN DERIVATIVE TO HUMAN SERUM ALBUMIN

Abstract Dialysis of hematoporphyrin derivative fraction A (HpD-A) off human serum albumin at 38°C followed the Hill equation for cooperative binding with saturation at 5 to 8. 600 dalton porphyrin units. Approximately 15% of the HpD-A was free for concentrations typical of human serum in photoradiation therapy. Possible structures of the tumor-localizing and -photosensitizing component in HpD-A are considered. Of these, a folded-over, covalent dimer appears to be more consistent with the photophvsical properties.     

THE MECHANISM OF ENERGY TRANSFER FROM POLY-p-BENZOYLPHENYLACETIMIDO-BOVINE SERUM ALBUMIN TO SMALL-MOLECULE QUENCHERS

Abstract— Results of a quantitative photochemical study of poly- p -benzoylphenylacetimido-bovine serum albumin in the presence of small-molecule triplet quenchers are reported. The efficiency of quenching by organic salts containing low triplet energy chromophores is shown to be qualitatively dependent on their predicted association constants to the modified protein. In addition, quenching is inhibited by salts of organic acids which possess high binding affinities for the protein but do not contain chromophores of low triplet energy. Quantitative treatment of the quenching and inhibition data yields results which strongly support the operation of an 'affinity controlled' mechanism for triplet energy transfer from the benzophenone moieties of the modified-bovine serum albumin to quenchers such as α-naphthylacetate and trans -cinnamate.     

PHOTOREACTIONS OF MACROCYCLIC DYES BOUND TO HUMAN SERUM ALBUMIN

The photophysical properties of tetrakis(4-sulfonatophenyl)porphyrin (H2TSPP), its tin (IV) complex (SnTSPP), aluminium(III) trisulfonatophthalocyanine (AIPCS), and the corresponding zinc(II) complex (ZnPCS), have been measured in H2O, D2O, and upon binding to human serum albumin (HSA). The triplet excited states of the various macrocyclic dyes generate singlet molecular oxygen, O2(1 delta g) in high quantum yield upon illumination in O2-saturated solution, even in the presence of HSA. The triplet states also abstract an electron from 4-aminophenol, forming the radical anion of the macrocycle. Quenching rate constants and quantum yields have been measured for the various processes in the presence and absence of HSA. It is found that HSA binds all the dyes at nonspecific sites close to the interface in such a manner that the dyes remain accessible to species residing in the solution phase. Dyes that do not possess axial ligands complexed to the central cation (e.g. H2TSPP, ZnPCS) are able to bind also at a deeper, more specific site on the protein where they are protected from species in solution. Under such conditions, triplet quenching by 4-aminophenol is restricted to long-distance electron tunnelling, for which the rate is relatively slow.     

THERMODYNAMICS OF PORPHYRIN BINDING TO SERUM ALBUMIN: EFFECTS OF TEMPERATURE, OF PORPHYRIN SPECIES and OF ALBUMIN-CARRIED FATTY ACIDS

Abstract Porphyrin binding to serum albumin was studied at the molecular level probing the effects of: porphyrin self-aggregation, porphyrin species, temperature and protein-bound fatty acids. Human serum albumin was found to have a single high-affinity site for porphyrin monomers, with binding constants of 2 x 10⁶, 5 x 10⁷ and 3 x 10⁸ (37^o C, neutral pH, M ⁻¹), for hemato-, deutero- and protoporphyrins, respectively. Three equilibria models for the dimer binding were developed and tested. The data were found to fit best with a model proposing a single high-affinity binding site for the dimer, independent of and different than the monomer site. The binding constants of the hematoporphyrin and deuteroporphyrin dimers to human serum albumin (37^o C, neutral pH, M^−l) being 4 x 10* and 5 x 10⁸ respectively. The temperature dependence (Dp and HSA, 22-37^o C) of the monomer binding showed the process to be entropy-driven (δG^o= -45 kJ mol⁻¹; δS^o=+146 kJ mol⁻¹; δH^o= 0 kJ mol⁻¹). For the dimer binding, the enthalpy change was found to be highly temperature-dependent implying continuous changes in the heat capacity of the system over the entire temperature range, the trend at the 37^o C region fitting an entropy-driven process. The monomer vs dimer differences in temperature dependence strongly support separate and independent binding sites for these species. Similar thermodynamics were determined for fatty-acid carrying as well as for fatty-acid free HSA, with mild quantitative (but not qualitative) shifts.     

放射标记法研究壳聚糖与牛血清白蛋白的自组装超薄膜

基片在两种带有相反电荷的聚电解质溶液中交替吸附 ,其表面形成致密有序的超薄膜的自组装 (ＥＳＡ ｅｌｅｃｔｒｏｓｔａｔｉｃｓｅｌｆ ａｓｓｅｍｂｌｙ)技术是由Ｄｅｃｈｅｒ及其合作者在 1 991年提出[1] ,由于简单易行 ,从一出现就受到了广大研究者的极大兴趣[2～ 4 ] .对生物材料来说 ,这无疑是一项非常重要且方便的表面改性手段 .因为生物材料在生物体内种植时 ,是否会被机体视为异物 ,关键在于机体与材料表面的相互作用 ,而与材料的本体性质基本无关[5] .因此利用这种技术 ,可对生物材料 ,特别是对那些生物相容性不好的材料表面进行…     

FLUORESCENCE INVESTIGATIONS OF ALBUMIN FROM PATIENTS WITH FAMILIAL DYSALBUMINEMIC HYPERTHYROXINEMIA*

Familial dysalbuminemic hyperthyroxinemia (FDH) is an autosomal dominant syndrome in which clinically euthyroid patients have elevated total thyroxine levels. These high serum thyroxine levels are traceable to altered binding of thyroxine to the patient's albumin. Albumin from FDH patients and normal volunteers have been purified. Reverse-phase and ion-exchange high performance liquid chromatography and sodium dodecyl sulfate-polyacrylamide gel electrophoresis on the FDH-human serum albumin (HSA) samples show a single band that comigrates with normal HSA. In both protein solutions the intrinsic fluorescence, upon 280 nm excitation, is predominantly due to the single tryptophan residue. The quantum yield of this intrinsic fluorescence in the FDH-HSA solutions is, however, reduced relative to that of HSA. Furthermore, the “average” lifetime value of the tryptophan emission in the FDH-HSA sample is less than that of normal HSA, consistent with its reduced quantum yield. The binding of thyroxine to both albumins effectively quenches the tryptophan emission probably via a nonradiative energy transfer mechanism. Time-resolved data suggest that the albumin from the dysalbuminemic patients is actually an approximately equimolar mixture of normal HSA and FDH-HSA indicative of heterologous expression. Quenching of the intrinsic HSA and FDH-HSA fluorescence by serial additions of thyroxine showed enhanced quenching of FDH-HSA relative to HSA at any T4 to albumin mole ratio, therefore supporting earlier reports of increased thyroxine affinity to FDH-HSA.     

FLASH PHOTOLYSIS OF BOVINE SERUM ALBUMIN: IDENTIFICATION AND DECAY KINETICS OF TRANSIENT INTERMEDIATES

Abstract. Using the method of flash photolysis, the triplet of the single indole side chain of human serum albumin was detected at room temperature. In a nitrogen saturated solution, this species was found to decay exponentially for over a factor of ten with a lifetime τ 0.5 ms. Analogous experiments, reported here, with bovine serum albumin yield a non-exponential decay which may be decomposed into two components. The yield of the longer lived triplet, with an average τ of ∼6 ms, is significantly enhanced by addition of a 20 fold excess of sodium dodecyl sulfate or 1 M Br^-. The yield of the shorter lived triplet, τ 0.4 ms, is unaffected by these treatments as was previously observed for the single indole in HSA. Thus, the short lived triplet may be assigned to the indole in BSA which is homologous to the one in HSA. The longer lived triplet may be assigned to the remaining indole of BSA. On the bases of wavelength dependence studies, two additional transients may be identified; the electron adduct of the disulfide bond, λ; 420 with a τ 30 ms, and the neutral indole radical,λ; 520 nm with τ ls. These results suggest that the triplet, because of its long τ, will be a valuable intrinsic reporter group for the study of the structure and dynamics of proteins in solution at room temperature.     

QUANTUM YIELD and EQUILIBRIUM POSITION OF THE CONFIGURATIONAL PHOTOISOMERIZATION OF BILIRUBIN BOUND TO HUMAN SERUM ALBUMIN*

Abstract— At low fluence rates it is possible to observe a photoequilibrium between Z,Z-bilirubin(BR) and its E isomers(collectively called PBR) bound to human serum albumin(HSA).For excitation centered at 465 nm, the fraction of PBR/HSA in the photoequilibrium mixture was observed to be 0.22 + 0.02. The quantum yield for conversion of BR/HSA to PBR/HSA was found to be 0.20 0.02. The equality of the quantum yield value and the fraction of PBR/HSA in the photoequilibrium mixture is consistent with a simple mechanism for the photoisomerization in which optically excited singlet states of BR and PBR convert rapidly and with virtually total efficiency to a common excited intermediate with twisted geometry that subsequently decays to BR and PBR in the ratio 4:1, respectively. Quantum yields for other photoprocesses of BR bound to HSA are much lower than that for configur-ational isomerization. The central role suggested for configurational isomerization in the phototherapy for neonatal hyperbilirubinemia is supported by these observations.     

RELATIVE CONTRIBUTIONS OF TRYPTOPHAN and TYROSINE TO THE PHOSPHORESCENCE EMISSION OF HUMAN SERUM ALBUMIN AT LOW TEMPERATURES

Abstract— Phosphorescence emission and excitation spectra, as well as decay profiles of human serum albumin, were investigated in the wavelength regions of the tryptophan and tyrosine absorption and emission spectra in potassium phosphate buffer at 77 K. Emission and excitation spectra were found to be linear superpositions of the contributions of the tryptophan and tyrosine residues. It is suggested, therefore, that there is no significant tyrosine to tryptophan energy transfer in this protein at low temperature. The phosphorescence decay is, in general, multiexponential with lifetime components of 5.95, 2.7, and 1.2 s. The longest lifetime is characteristic of tryptophan, whereas the two short components are attributed to two types of tyrosine residues located in different environments within the protein. The latter is confirmed by a detailed analysis of the phosphorescence decay profiles determined at different emission wavelengths, and utilizing different wavelengths of excitation favoring either the tryptophan or tyrosine residues.     

染料壳聚糖微球的制备及其对人血清白蛋白吸附性能研究

人血清白蛋白(Human Serum Albumin,HSA)是血浆中含量最丰富的蛋白质,约占血浆总蛋白的60%.在人体内,HSA有许多重要的生理功能[1],临床上广泛应用于手术输血和危重病人补液,治疗创伤休克、烧伤、水肿和低白蛋白血症等,而且能增强人体抵抗能力,是迄今为止产量最大、临床用量最大     

PROPERTIES OF THE ULTRAVIOLET-LIGHT-MEDIATED BINDING OF BOVINE SERUM ALBUMIN TO DNA*

Abstract— The binding of DNA to protein mediated by U V (254 nm) radiation has been investigated using binding of the complex to Millipore membrane filters as an assay technique. The reaction proceeds through an activated protein intermediate which then reacts with the DNA. The activated protein has a half-life of about 75 min at 0°C and about 18 min at 37°C. Short wavelengths are more efficient in forming the complex than wavelengths in the 250–280 nm range. N-ethyl maleimide treatment of protein before irradiation markedly inhibits the reaction.     

DRUG SENSITIZATION: PHOTOBINDING OF SULFANILAMIDE TO BOVINE SERUM ALBUMIN

Abstract— Photobinding of sulfanilamide to bovine serum albumin (BSA) was investigated by irradiating BSA and buffered BSA/drug solutions with UV light (Λ= 300 nm) under anaerobic conditions. The protein solutions were then denatured and the unbound sulfanilamide removed. Marked differences in the UV and fluorescence spectra of the solutions before and after irradiation were observed, suggesting covalent binding of the drug to BSA. This was confirmed using [¹⁴C]labelled sulfanilamide. The extent of photobinding of sulfanilamide determined using the radiolabeled drug, was concentration dependent. The binding ratio varied from 3 mol drug per mol BSA for a 10^-4 M drug concentration, to 10 mol drug per mol BSA for 10^-2 M drug concentration.
The protein solutions were hydrolysed under acid conditions and the amino acids obtained were analysed by ion exchange chromatography. The hydrolysate of irradiated BSA (10^-4 M ) -sulfanilamide (10^-2 M ) mixture lost about 10 mol of cystine per mol of BSA. This loss was not observed after hydrolysis of irradiated alone or non-irradiated BSA. Irradiation of cystine with [¹⁴C]sulfanilamide in HC1 solutions produced the same compound as was found after hydrolysis of irradiated BSA/sulfanilamide mixtures. This was demonstrated by autoradiography of paper chromatograms. The same compound was also detected in an irradiated [³⁵S]cystine non-labelled sulfanilamide mixture. It was not detected, however, after irradiation of a mixture of all amino acids of BSA excluding cystine. These data suggest that cystine residues are involved in the photobinding of sulfanilamide (or its photoproducts) to BSA.