胞嘧啶核苷键联卟啉的合成及其与牛血清白蛋白的相互作用

基于卟啉化合物的光敏性和对肿瘤细胞有特殊的亲和力以及核苷类化合物的抗肿瘤及抗癌活性, 设计合成了胞嘧啶核苷卟啉化合物6和8, 其结构由¹H NMR, IR, UV-Vis, MS 和元素分析表征. 同时, 利用荧光光谱考察了上述核苷卟啉与牛血清白蛋白(BSA)的相互作用, 结果表明它们对BSA荧光有较强的静态猝灭作用.     

Hydrophobic Volume Effects in Albumin Solutions

Density measurements of aqueous albumin solutions as a function of concentration and temperature are reported. The solvents were H(2)O, D(2)O, and a physiological H(2)O-based buffer. An anomaly of the density at very small concentrations of albumin in D(2)O was found. Furthermore, the partial specific volume of albumin is remarkably different in D(2)O and H(2)O. We attribute both effects to structural differences of the solvents. Copyright 2001 Academic Press.     

Hydrophobic Interaction Between Domain I of Albumin and B Chain of Detemir May Support Myristate-Dependent Detemir-Albumin Binding

The bindings of detemir [LysB29(Nε-tetradecanoyl)des(B30)-insulin] with two highly homologous albumins, HSA (human serum albumin) and BSA (bovine serum albumin), were investigated through CD, spectrofluorophotometry, and molecular docking analysis. The absence of any tryptophanyl residue in detemir makes albumin binding study possible by exclusive tryptophanyl spectral quenching at 340 nm (λem = 296 nm). The interactions found to be static (Kq > 10¹⁰ M^?1 s^?1) with Stern–Volmer constants ≈10³ M^?1. The observed ΔG ⁰ that was negative in all cases concludes the reactions were spontaneous. Domains I and III of an albumin unfold with 5.0 M urea at pH 7.4, although domain II remains intact. Significant decreases in ΔH ⁰ and ΔS ⁰ were due to unfolding explicit that detemir binding may involve domains I and III of albumins. Temperature-dependent changes in binding were higher in HSA than BSA but after unfolding such changes were very less, further indicating the role of domains I and III in detemir binding. Pro28 and Tyr26 of insulin were found to be interacting with Arg114 and Val116 of HSA domain I, while myristate segment of detemir binds to Lys519 of domain III. Interactions seem to be predominantly hydrophobic and entropy driven. Although detemir binds to albumin through myristate, the peptide part shows involvement in binding.     

金属元素组与血清白蛋白的竞争结合反应性能研究

利用亲和毛细管电泳（Affinitycapillaryelectrophoresis,ACE）法研究金属元素组和血清白蛋白（Bovineserumalbumin,BSA）的竞争结合反应性能。基于位点结合模型,构建双金属组[Zn²⁺,Cu²⁺]与血清白蛋白结合反应模型,建立多元金属组与生物大分子竞争结合的理论方程,测定结合参数并解析动力学机制。结果表明,金属元素组[Zn²⁺,Cu²⁺]与BSA发生竞争结合反应形成配合物Zn²⁺-BSA和Cu²⁺-BSA。依据有效淌度变化,通过建立的理论方程非线性拟合竞争结合反应的平均表观结合常数K_Zn²⁺-BSA=4.01×10⁴L·mol^-1、K_Cu²⁺-BSA=7.75×10⁴L·mol^-1。结合反应均为快平衡反应,Cu²⁺对Zn²⁺离子的结合作用有明显拮抗作用。分析ACE谱显示配合物的峰高与配体结合能力大小、配合物稳定性之间存在量效关系。     

金属元素组与血清白蛋白的竞争结合反应性能研究

利用亲和毛细管电泳(Affinity capillary electrophoresis,ACE)法研究金属元素组和血清白蛋白(Bovine serum albumin,BSA)的竞争结合反应性能。基于位点结合模型,构建双金属组[Zn2+,Cu2+]与血清白蛋白结合反应模型,建立多元金属组与生物大分子竞争结合的理论方程,测定结合参数并解析动力学机制。结果表明,金属元素组[Zn2+,Cu2+]与BSA发生竞争结合反应形成配合物Zn2+-BSA和Cu2+-BSA。依据有效淌度变化,通过建立的理论方程非线性拟合竞争结合反应的平均表观结合常数KZn2+-BSA=4.01×104L·mol-1、KCu2+-BSA=7.75×104L·mol-1。结合反应均为快平衡反应,Cu2+对Zn2+离子的结合作用有明显拮抗作用。分析ACE谱显示配合物的峰高与配体结合能力大小、配合物稳定性之间存在量效关系。     

Binding Interaction of Xanthoxylin with Bovine Serum Albumin

Three independent techniques have been used to investigate the interaction between bovine serum albumin (BSA) and xanthoxylin (XT). UV-Vis absorption spectroscopy measurements showed that there is a XT-BSA complex formed with an overall binding constant of K=1.01×10⁵ L⋅mol⁻¹. Spectroscopic techniques including synchronous fluorescence and Fourier transform infrared (FT-IR) were used to assess the structural effects of XT binding on BSA. The FT-IR experiments showed that there is a decrease of the amount of α-helix from 50.2 to 48.1% and an increase of the β-sheet from 32.9 to 36.9% in the XT-BSA complex. In addition, XT binds to site I of the protein with a distance of 2.07 nm between tryptophan residues and XT.     

Interaction of Cationic Manganese Porphyrins with DNA. A Binding Model

The DNA cleavage properties of two cationic manganese porphyrins possessing different peripheral substituents were compared. The identical nature of the strand scission patterns of the porphyrins on a 139 base pair restriction fragment of pBR-322 DNA, along with other evidence, suggests that the porphyrin is end-on bound via the minor groove in a melted or partially melted region of DNA. This unusual binding mode underscores the potential of outisde binding cationic metalloporphyrins as probes for low melting regions of DNA     

水杨酸键联卟啉的合成及与牛血清白蛋白的相互作用

以溴代烷氧基苯基卟啉(1)为原料与水杨酸作用,分别得到了化合物2和3,再与醋酸钴反应,得到了钴卟啉配合物4和5.新化合物分别由¹HNMR,IR,UV-Vis,MS和元素分析确证.同时,利用荧光光谱考察了金属卟啉与牛血清白蛋白的相互作用.     

新型尾式水杨酸卟啉的合成及其与牛血清白蛋白的相互作用

以吡咯、苯甲醛和对羟基苯甲醛为原料,经一锅法制得5-(4-羟基苯基)-10,15,20-三苯基卟啉(1);1与直链二溴烷烃反应制得溴代烷氧基卟啉(3a~3e);3a~3e分别与水杨酸经消除反应合成了10个尾式水杨酸卟啉4a~4e和5a~5e,其中4a,4b,4d,4e,5a,5b,5d和5e为新化合物,其结构经UV-Vis,1H NMR,IR和ESI-MS表征。用荧光光谱研究了4a~4e和5a~5e与牛血清白蛋白(BSA)的相互作用。结果表明:4a~4e和5a~5e对BSA的荧光猝灭为静态猝灭;Stern-Volmer曲线的线性关系良好;kq值均远大于2.0×1010L·mol-1·s。     

Synthesis of Metal Porphyrins Tailed with Salicylic Acid and their Interaction with Bovine Serum Albumin

A synthetic method of porphyrins tailed with salicylic substituents is described.Reaction of bromoalkoxyphenyl porphyrin 1 with salicylic acid gave porphyrins 2-5. These new compounds were confirmed by ^1H NMR, IR, UV-vis, MS and elemental analysis, and observed their interaction with bovine serum albumin (BSA) in fluorescence spectrum.     

Binding of Dioxopromethazine Hydrochloride with Human Serum Albumin and Its Effect on the Conformation of the Protein

The interaction between dioxopromethazine hydrochloride (DPZ) and human serum albumin (HSA), in vitro, was investigated by means of fluorescence, absorption and circular dichroism (CD) spectroscopy. The results obtained from analysis of the fluorescence spectra indicate that DPZ has a strong ability to quench the intrinsic fluorescence of HSA through a static quenching mechanism. The HSA?CDPZ binding distance was determined to be less than 7?nm, suggesting that energy transfer from HSA to DPZ may occur. The thermodynamic parameters of the interaction between DPZ and HSA were measured according to the van??t Hoff equation. The negative enthalpy change (??H ⁰) and positive entropy change (??S ⁰) values indicate that hydrophobic and electrostatic interactions play major roles in the binding between DPZ and HSA. The binding process was a favorable process in which the Gibbs energy change (??G ⁰) is negative. The results of displacement experiments suggested that DPZ is located in site I of HSA within subdomain IIA. In addition, the results of absorption, synchronous fluorescence and CD spectra show that binding of DPZ with HSA can induce conformational changes in HSA.     

Adsorption of Bovine Serum Albumin and Lysozyme on Hydrophobic Calcium Hydroxyapatites

The adsorption of bovine serum albumin (BSA) and lysozyme (LSZ) to oleyl phosphate(OP)-grafted calcium hydroxyapatite (OP-CaHAP) with different degrees of hydrophobicity, ranging the number of surface oleyl group per unit nm2 (nO) from 0 to 2.60, was investigated. The pronounced effects of the hydrophobic moiety of adsorbent on protein adsorption were observed. The saturated amount of adsorbed BSA (ns) was increased up to nO = 0.6 by an enlargement of hydrophobic interaction between hydrophobic CaHAP particle and proteins. However, ns decreased at nO >/= 1.3 by increasing the electrostatic repulsive force between negatively charged BSA and OP-CaHAP particles. On the other hand, the ns value of LSZ was continuously increased up to nO = 2.0 and saturated by increasing either the hydrophobic interaction or the electrostatic attraction of positively charged LSZ and negatively charged OP-grafted CaHAPs. The BSA adsorption experiment revealed that the effect of positively charged adsorption sites on the exposed ac or bc crystal faces (C-sites) of the CaHAPs is screened by the OP-groups grafted on their particle surfaces. Copyright 1999 Academic Press.     

抗菌素痢菌净与牛血清白蛋白相互作用的光谱研究

用荧光光谱和紫外吸收光谱法研究了抗菌素痢菌净(MEQ)与牛血清白蛋白(BSA)的相互作用。讨论了荧光猝灭机理,结果表明是动态猝灭过程;计算了不同温度下的猝灭常数和热力学参数。MEQ与BSA的相互作用为一个由熵驱动的自发过程,疏水作用力也起重要作用。由FRET能量转移理论计算得出了MEQ与BSA结合位置的距离r=4.5 nm。应用同步荧光和三维荧光研究了BSA在MEQ存在或不存在时的构象变化,结果表明：MEQ对BSA构象的影响不大。     

咪唑型离子液体与牛血清蛋白的缔合特性

通过紫外-可见光谱、荧光光谱、同步荧光光谱、圆二色谱、衰减全反射红外光谱、负染-透射电镜、等温滴定微量热等实验方法系统地探讨了咪唑型离子液体与牛血清蛋白(BSA)的缔合特性.结果发现,离子液体[Bmim]Cl的加入使得BSA的紫外吸收强度增加,同时也会导致其荧光猝灭,并且这种猝灭是静态猝灭.同步荧光的研究结果表明,[Bmim]Cl分子可与蛋白质中接近色氨酸残基的区域发生相互作用,使蛋白质的构象和内部的疏水结构发生改变;负染色法透射电镜直观地显示了加入离子液体后形成的蛋白质-离子液体复合物结构逐渐变大;圆二色谱和衰减全反射红外光谱表明:在离子液体与BSA缔合过程中,离子液体的加入使得BSA二级结构中的α-螺旋和β-折叠的含量降低,从而引起蛋白质二级结构的变化;表面张力法和等温滴定微量热法进一步证实上述缔合作用为静电作用和疏水作用共同作用的结果,但离子液体的烷基链与BSA疏水内腔之间的疏水作用是离子液体与BSA缔合的主要驱动力.     

Unusual Binding of a Potential Biomarker with Human Serum Albumin

This study investigates the specific binding of a potential biomarker, [2,2′‐bipyridyl]‐3,3′‐diol (BP(OH)₂), with human serum albumin (HSA). The binding of BP(OH)₂ at the two primary drug‐binding sites on HSA (Sudlow′s sites I and II) is explored by a competitive‐binding study and monitored by considering the green‐light emission from its diketo tautomer. Warfarin is used as a marker for site I and dansyl‐L ‐proline (DP) as a competitor for site II. Steady‐state and time‐resolved fluorescence measurements affirm that neither of Sudlow′s sites is the binding locus of BP(OH)₂. To gain an idea regarding the probable binding site of BP(OH)₂, we perform molecular‐docking studies, which reveal a close proximity of the probe to Trp‐214 in subdomain IIA of HSA. Confirmation of this contention is achieved by studying the quenching of the fluorescence of Trp‐214 in the presence of BP(OH)₂. Moreover, static quenching seems to be responsible for the depletion of the fluorescence of Trp‐214, as manifested by the invariance of the intrinsic fluorescence lifetime of Trp‐214, as a function of the concentration of BP(OH)₂. Based on displacement and quenching studies, supported by molecular docking, we propose that BP(OH)₂ binds in a cleft that separates subdomains IIIA and IIB, which is in close proximity to Trp‐214.     

甲磺酸培氟沙星与人血清白蛋白之间结合模式的研究

采用实验和计算的方法研究了甲磺酸培氟沙星与人血清白蛋白之间的结合作用.荧光法测得甲磺酸培氟沙星与人血清白蛋白形成一种类型的复合物,结合常数为1.7×10⁵ L&;#8226;mol^－1,有1.05个平均结合位点；微量热法测得该药物-蛋白结合过程中焓变为1.03 kJ&;#8226;mol^－1,熵变为101.28 J&;#8226;K^－1&;#8226;mol^－1,反应为熵驱动.用分子对接的方法预测了甲磺酸培氟沙星与人血清白蛋白的结合模式.计算表明,甲磺酸培氟沙星可结合在人血清白蛋白的两个药物结合位点,疏水作用即熵效应在药物与蛋白的结合中起重要作用,预测的结合自由能和实验值基本一致.     

Application of Supermacroporous Monolithic Hydrophobic Cryogel in Capturing of Albumin

Supermacroporous poly{2-hydroxyethyl methacrylate-co-[N,N-bis(2,6-diisopropylphenyl)-perylene-3,4,9,10-tetracarboxylic diimide]} [poly(HEMA-co-DIPPER)] monolithic cryogel column was prepared by radical cryocopolymerization of HEMA with DIPPER as functional comonomer and N,N′-methylene-bisacrylamide (MBAAm) as crosslinker directly in a plastic syringe for adsorption of albumin. The monolithic cryogel contained a continuous polymeric matrix having interconnected pores of 10–50 μm size. Poly(HEMA-co-DIPPER) cryogel was characterized by swelling studies, FTIR, scanning electron microscopy, and elemental analysis. The equilibrium swelling degree of the poly(HEMA-co-DIPPER) cryogel was 14.7 g H₂O/g dry cryogel. Poly(HEMA-co-DIPPER) cryogel was used in the adsorption/desorption of albumin from aqueous solutions. The nonspecific adsorption of albumin onto plain poly(HEMA) cryogel was very low (3.36 g/g polymer). The maximum amount of albumin adsorption from aqueous solution in acetate buffer was 40.9 mg/g polymer at pH 5.0. It was observed that albumin could be repeatedly adsorbed and desorbed with the poly(HEMA-co-DIPPER) cryogel without significant loss of adsorption capacity.     

A Thermodynamic Study on the Binding of Human Serum Albumin with Lanthanum Ion

Thermodynamics of the interaction between lanthanum(III) ion, La³⁺, and human serum albumin (HSA), was investigated at pH 7.0 and 300 K in Tris‐HCl buffer by isothermal titration calorimetry. A solvation model was used to reproduce the enthalpies of HSA interaction with La³⁺. The solvation parameters recovered from our new model were attributed to the structural change of HSA and its biological activity. The interaction of HSA with La³⁺ showed a set of two binding sites with negative cooperativity.     

Anion Binding Properties of N-Confused Porphyrins at the Peripheral Nitrogen

Ni(II), Pd(II), and Cu(II) complexes of N-confused porphyrin (NCP) exhibit anion binding properties through a hydrogen bonding interaction at the peripheral NH of confused pyrrole ring. The binding constants of the tetrakis(pentafluorophenyl)-NCP metal complexes (1-M, M= Ni, Pd, Cu) for various halide anions in CH₂C1₂ increase in the order of F^? > Cl^? > Br^? > I^?, respectively. Zwitterionic resonance form of the NCP complexes as well as interactions between halide anions and a pentafluorophenyl group are suggested to be important for efficient anion binding.