牛血清蛋白质三维有序大孔材料

用胶体晶体为模板制备了牛血清白蛋白和异硫氰基荧光素标记的牛血清白蛋白的三维有序大孔材料. 表征了孔材料的结构和荧光发射光谱. 表明所制备的孔材料具有规整的三维有序孔结构, 荧光素标记的牛血清白蛋白三维有序大孔材料具有良好的荧光发射性质.     

褐藻多糖铈配合物对质粒DNA及牛血清白蛋白的裂解作用

以褐藻糖胶、褐藻酸及褐藻演粉为配体，分别与四价的铈（Ce^4 ）结合，形成了水溶性的褐藻多糖铈配合物，在生理中性条件下，它们对牛血清白蛋白（BSA）均有一定的裂解作用，但对质粒DNA（Plasmide DNA）仅有褐藻淀粉铈配合物有非常明显的裂解作用。     

Interaction of Nicotine and Bovine Serum Albumin

Nicotine. 3-(l-methyl-2-pyrrolidinyl) pyridine, is a major alkaloid in tobacco products.typically composing l-2% weight of tobacco. So far, there are a 'great deal of papersreporting the effect of nicotine on various biological tissues of animals and humans. Thepharmacological effect of nicotine is a dominant addiction factor for smoking. Since avery large population is frequently exposed to nicotine through the mainstream and/orsidestream of smoking inhalation, the interaction of nicotine wit…     

荧光素与牛血清蛋白的作用及其分析应用

１引言根据染料与蛋白质的相互作用建立测定蛋白质的分析方法已有不少报道,但寻找简便、快速、准确的测定蛋白质的分析方法仍然是人们研究的热点。生物大分子与小分子配体相互作用的研究,目前多用透析,超滤或凝胶色谱等实验方法。当小分子配体与生物大分子结合前后的吸收光谱有一定差别时,用光度法在不经分离的情况下进行研究比上述方法要简便得多,且实验得信息较为可靠。本文正是利用荧光素与ＢＳＡ相互作用形成复合物最大吸收峰的波长４８０ｎｍ,比试剂本身红移约９ｎｍ,提出的分析方法,线性范围宽,灵敏度高,方法简便、快速,干…     

单宁微球对牛血清蛋白的吸附

采用反相悬浮聚合法制备单宁微球,利用扫描电子显微镜对微球的表面形貌进行观察.同时以单宁微球为吸附剂,探讨pH值、单宁微球质量、牛血清蛋白起始浓度、吸附时间等条件对单宁微球吸附牛血清蛋白性能的影响,得出单宁微球吸附牛血清蛋白的最佳条件.并用两种动力学模型进行拟合.结果表明,单宁微球对牛血清蛋白的吸附速率先快后慢,最后吸附...     

Interaction Between Surfactin and Bovine Serum Albumin

The interaction of surfactin, a typical biosurfactant, with bovine serum albumin (BSA) was investigated by surface tension, fluorescence, freeze-fractured transmission electron microscopy (FF-TEM) and circular dichroism (CD) measurements. The surface tension curves of pure surfactin solution and surfactin/BSA solutions have different phenomena, where two obvious inflections determined as the critical aggregation concentration (cac) and the critical micelle concentration (cmc) appear for surfactin/BSA solutions. The higher BSA concentration, the higher cac and cmc values for surfactin/BSA solution. Fluorescence spectra show that the structure change of BSA is dependent on both surfactin and BSA concentration. The micropolarity, FF-TEM and CD results further demonstrate the interaction between BSA and surfactin. The excess free energy (ΔG⁰) of surfactin/BSA interactions have been obtained as ?6.13 and 5.32 kJ/mol for 1.0 × 10^?6 and 3.8 × 10^?6 mol/L BSA concentration, respectively. The binding ratio (R) determined for surfactin/BSA systems are higher than that reported for dirhamnolipid to BSA. Above all, it can be concluded that the hydrophobic interaction and the hydrogen bonds between surfactin and BSA play the key role for the high binding ratio for surfactin to BAS.     

蒂巴因与牛血清蛋白的相互作用

用荧光光谱和紫外-可见吸收光谱研究了中性条件下蒂巴因与牛血清白蛋白(BSA)结合反应的光谱行为,发现蒂巴因对BSA有较强的荧光猝灭作用,且蒂巴因的紫外吸收光谱和BSA的荧光发射光谱有一定程度的重叠,据此求得了其结合反应的结合位点数为1,结合常数为3.76×105,作用距离2.95 nm,并通过求算的基本热力学参数推测1分子的蒂巴因与1分子的蛋白质的212位色氨酸以静电作用力结合.     

Interaction between Xanthoxylin and Bovine Serum Albumin

在模拟生理条件下,采用荧光光谱法、圆二色光谱法和红外光谱法研究了花椒油素(XT)与牛血清白蛋白（BSA）的相互作用。结果表明花椒油素与牛血清白蛋白之间发生动态和静态联合猝灭,二者间的的猝灭常数(K)在286, 298和310 K分别为3.31 × 105, 到2.03 × 105 和 0.94 × 105 L∙mol-1. 热力学参数表明, 花椒油素与牛血清白蛋白间以疏水作用力为主。圆二色光谱和红外光谱法表明加入花椒油素后,牛血清白蛋白的二级结构发生了变化,其中α-螺旋减少了3.9%。另外,我们还研究了共存离子对两者结合的影响。     

恩诺沙星与牛血清白蛋白的相互作用

恩诺沙星与牛血清白蛋白的相互作用;恩诺沙星;牛血清白蛋白;荧光猝灭     

吡蚜酮与牛血清白蛋白的相互作用

利用紫外吸收、荧光、同步荧光光谱及圆二色谱研究了吡蚜酮与牛血清白蛋白(BSA)的相互作用. 结果发现, 吡蚜酮使BSA的紫外吸收峰强度降低, 峰位红移; BSA的特征荧光峰猝灭, 荧光猝灭常数KSV随着温度的升高而降低, 表明吡蚜酮与BSA发生了较强的相互作用, 且吡蚜酮对BSA的荧光猝灭机制属于静态猝灭. 计算了不同温度下的结合常数和结合位点数; 由van′t Hoff方程计算出体系的ΔH和ΔS值, 得出二者之间的作用力主要为氢键和范德华力; 根据非辐射能量转移理论确定了给体-受体间的结合距离r=2.4 nm. 采用同步荧光光谱和圆二色谱考察了吡蚜酮对牛血清白蛋白构象的影响.     

1-萘酚诱导人血清白蛋白和牛血清白蛋白构象的变化

采用稳态荧光光谱、同步荧光光谱、荧光共振能量转移技术结合分子对接法,探究了1-萘酚(1-OHNap)诱导人血清白蛋白(HSA)和牛血清白蛋白(BSA)构象变化的差异.结果 表明,与1-OHNap的结合作用使HSA中荧光团周围微环境极性发生改变,BSA中Trp残基周围微环境的极性增加;同时,与1-OHNap的结合作用使H...     

变色酸与牛血清白蛋白的相互作用

采用荧光光谱法和紫外-可见分光光度法研究了变色酸与牛血清白蛋白之间的相互作用。结果表明:变色酸对牛血清白蛋白有较强的荧光猝灭作用。根据Stern-Volmer方程得到了荧光猝灭常数,并判断由于与变色酸反应而导致牛血清白蛋白的荧光猝灭属于静态猝灭。采用Lang-muir单分子吸附模型计算了结合常数和结合位点数。从计算得到的热力学参数ΔH和ΔS推断了变色酸与血清白蛋白反应的作用力为氢键和范德华力。     

牛血清白蛋白的光损伤和光氧化机理

运用激光闪光光解瞬态吸收技术, 在266 nm激光激励下, 研究了牛血清白蛋白(BSA)光损伤和被SO4-·单电子氧化的反应机理, 表征了反应过程中生成的自由基. 结果表明, 在266 nm激光照射下, BSA可同时发生光电离和光激发, 生成色氨酸阳离子自由基(Trp/NH+·), 由Trp/NH+·快速脱质子形成的色氨酸中性自由基(Trp/N·)及色氨酸三重激发态(3Trp*), 3Trp*再与酪氨酸(Tyr)发生分子内电子转移生成酪氨酸中性自由基(Tyr/O·). 在SO4-·单电子氧化的反应中, 借助减谱技术, 求得BSA中Tyr和色氨酸(Trp)自由基的表观生成速率常数, 但未发现分子内电子转移现象, 阐明了SO4-·自由基是通过与BSA中的Tyr和Trp发生电子转移反应来氧化BSA的, SO4-·氧化BSA的反应速率常数为1.51×10¹⁰ L·mol^-1·s^-1, 从而为进一步研究血清白蛋白的氧化还原代谢过程提供理论基础.     

靛蓝二磺酸钠和牛血清白蛋白的结合反应

用荧光光度法及吸光光度法研究了在PH 7.0的三(羟甲基)氨基甲烷-HCl缓冲溶液中靛蓝二磺酸钠(IDGS)与牛血清白蛋白(BSA)的相互结合反应.根据福斯特无辐射能量转移机理,求算了靛蓝二磺酸钠与牛血清白蛋白给体-受体间距离为3.63 nm,能量转移效率为0.44,临界能量距离为2.44 nm.靛蓝二磺酸钠与牛血清白蛋白的相互结合作用为静态和动态猝灭过程,其作用机制为能量转移机制.     

Competitive Process of Binding Between the Anionic Surfactants Sodium Dodecyl Sulfate and Sodium Cholate in Bovine Serum Albumin

Summary: In this study sodium cholate (NaC) was used as a representative bile salt for the competitive binding between NaC and sodium dodecyl sulfate (SDS) in bovine serum albumin (BSA), in 0.02 M tris-HCl buffer solution at pH 7.50 and 25 °C. The NaC and SDS associations with BSA were monitored at low surfactant concentrations where only this specific binding process can develop. The applied method to monitor the binding was based on the analysis of the effect of SDS and NaC concentrations and their mixtures upon the fluorescence intensity of the BSA tryptophan residues. This consists of the measurement of the surfactant monomer partitioning between the dispersion medium and the microaggregates on the protein molecule where the binding is indicated by the quenching of the fluorescence chromophores. Experimentally, varying the protein concentration, the surfactant concentration needed to reach a given I_o/I ratio (I_o and I are the intensities with and without protein, respectively) was measured. The analyses, based on the average number of surfactant molecules bound on the protein, indicated that the SDS is a more efficient quencher than the bile salt. The need for 4–6 NaC bound molecules to give the same protein quenching efficiency by a single molecule of SDS was estimated. We concluded that the differences in the competitive binding on the protein are exclusively related to the quenching efficiency in the formation of the nonfluorescent fluorophore-quencher complex via a physical contact and static quenching process.     

Dynamic Behaviors and Morphology Change of Anionic Phospholipid DPPG Monolayer Caused by Bovine Serum Albumin at Air-Water Interface

The interaction between bovine serum albumin (BSA) and the anionic 1.2-dipalmitoyl-snglycero- 3-(phospho-rac-(1-glycerol)) (sodium salt) (DPPG) phospholipid at different subphase pH values was investigated at air-water interface through surface pressure measurements and atomic force microscopy (AFM) observation. By analyzing surface pressure-mean molecular area (π-A) isotherms, the limiting molecular area in the closed packing state-the concentration of BSA (A_lim-[BSA]) curves, the compressibility coefficient-surface pressure (C_S^-1-π) curves and the difference value of mean molecular area-the concentration of BSA (ΔA-[BSA]) curves, we obtained that the mean molecular area of DPPG monolayer became much larger when the concentration of BSA in the subphase increased at pH=3 and 5. But the isotherms had no significant change at different amount of BSA at pH=10. In addition, the amount of BSA molecules adsorbed onto the lipid monolayer reached a threshold value when [BSA]>5×10^-8 mol/L for all pHs. From the surface pressure-time (π-t) data, we obtained that desorption and adsorption processes occurred at pH=3, however, there was only desorption process occurring at pH=5 and 10. These results showed that the interaction mechanism between DPPG and BSA molecules was affected by the pH of subphase. BSA molecules were adsorbed onto the DPPG monolayers mainly through the hydrophobic interaction at pH=3 and 5, and the strength of hydrophobic interaction at pH=3 was stronger than the case of pH=5. At pH=10, a weaker hydrophobic interaction and a stronger electrostatic repulsion existed between DPPG and BSA molecules. AFM images revealed that the pH of subphase and [BSA] could affect the morphology features of the monolayers, which was consistent with these curves. The study provides an important experimental basis and theoretical support to understand the interaction between lipid and BSA at the air-water interface.     

荷花碱与牛血清白蛋白的相互作用

利用多种光谱技术研究了在pH7.40的Tris-HCl缓冲体系下,荷花碱与牛血清白蛋白(BSA)的相互作用。研究发现荷花碱对牛血清白蛋白有较强的荧光猝灭作用且为静态猝灭。用Stern-Volmer和Line weaver-Burk方程处理荧光猝灭数据,得到反应的结合常数在293K时为1.70×104L/mol,结合的ΔH°=-20.2kJ/mol,ΔS°=12.0J/(K.mol)。该药物与血清白蛋白之间的作用力为疏水作用和静电作用。根据Frster非辐射能量转移理论求得荷花碱与BSA相互结合时,其供体-受体间的距离为2.59nm。用圆二色谱等手段表明结合对蛋白的构象产生了影响。同时考察了中药活性成分甘草次酸和脂肪酸对结合的影响。     

5-氟尿嘧啶与牛血清白蛋白的相互作用

根据合理的假设和Langmuir结合理论, 在298.15 K下, 以等温滴定微量热(ITC)实验数据为依据, 应用非线性最小方差拟合方法确定了抗肿瘤药物配5-氟尿嘧啶(5-FU)与牛血清白蛋白(BSA)相互作用的热力学性质的改变. 研究结果表明, 牛血清白蛋白(BSA)与5-氟尿嘧啶相互作用存在两类结合位点. 第一类结合, N=(54.0 0.3), ⊿H⁰=(30.0±0.4) kJ·mol^-1 (吸热), ⊿S⁰=(196.0±2.6) J·mol-1·K-1(熵增), ⊿G⁰=(-28.4±0.3) kJ·mol^-1; 第二类结合, N=(77.0±0.4), ⊿H⁰=(-20.0±0.4) kJ·mol^-1 (放热), ⊿S⁰=(28.6±0.3) J·mol^-1·K^-1 (熵增), ⊿G⁰=(-28.5±0.2) kJ·mol^-1. 结合体系的圆二色谱(CD)分析结果说明, 抗肿瘤药物5-氟尿嘧啶与BSA的相互作用诱导蛋白质(BSA)二级结构单元的相对含量发生了一定程度的变化.     

α-硫辛酸与牛血清白蛋白的相互作用

利用荧光光谱和紫外-可见吸收光谱研究了在缓冲溶液中不同温度下α-硫辛酸(ALA)与牛血清白蛋白(BSA)的相互作用。结果表明,ALA对BSA的内源荧光猝灭为静态猝灭过程,猝灭常数KSV分别为4.65×103L/mol(26℃)和4.46×103L/mol(37℃)。依据Frster非辐射能量转移机制,得到给体(BSA)-受体(ALA)间的结合距离r=2.90 nm,能量转移效率E=5%。测定了该反应在不同温度下的结合常数KA=4.31×103L/mol(26℃),4.27×103L/mol(37℃),以摩尔比1∶1结合。根据不同温度下的结合常数确定了相互作用过程的热力学参数,并根据热力学参数确定了ALA与BSA之间作用力主要是静电作用。