荧光探针法研究百草枯与DNA的相互作用

以中性红（NR）为分子探针,应用紫外光谱法和荧光光谱法研究了除草剂百草枯（PQ）与小牛胸腺DNA（ctDNA）之间的相互作用。在pH7.3的Tris-HCl（5×10-2mol.L-1）缓冲溶液中,NR分子主要以嵌插方式结合到ctDNA双螺旋结构上,百草枯的加入抑制了NR与ctDNA之间的结合,用Stern-Volmer方程进行数据处理,表明百草枯对ctDNA-NR的荧光猝灭不是单纯的静态或动态猝灭方式,属于混合型的。综合紫外光谱、离子强度等研究证实,在该实验条件下,百草枯与DNA之间存在静电和嵌插两种作用。     

荧光光谱法研究咖啡因与肌红蛋白的相互作用

采用荧光光谱法在生理pH 7.4条件下研究了药物咖啡因与肌红蛋白分子间的相互作用,表明这种相互作用能使肌红蛋白的内源荧光猝灭。通过猝灭常数,结合常数和结合位点数的计算,证明此猝灭为静态猝灭机制。咖啡因和肌红蛋白形成1∶1稳定配合物,形成常数(18 ℃)K_A=1.82×104 L·mol-1;根据热力学参数确定了它们之间的主要作用力为疏水力和静电力。利用同步荧光光谱法研究了咖啡因对肌红蛋白构象的影响。咖啡因能使肌红蛋白的构象发生改变,导致蛋白质分子中色氨酸和酪氨酸残基所处微环境由原来的疏水环境不同程度地向亲水环境转变。     

1-脱氧野尻霉素与人血清白蛋白相互作用的荧光光谱

在模拟生理条件下(pH 7.4),采用荧光光谱及傅里叶变换红外光谱研究了1-脱氧野尻霉素(1 -DNJ)与人血清白蛋白(HSA)之间的相互作用方式及机理.结果表明,1-DNJ对HSA的荧光猝灭作用主要为静态猝灭,两者之间形成了1∶1的复合物.通过计算获得了不同温度下的结合常数及结合位点数,并根据1-DNJ与HSA结合的热力学参数,确定了两者之间的主要作用力为疏水作用与静电引力.同步荧光光谱显示1-DNJ对HSA的构象产生了影响,并通过傅里叶变换红外光谱确定了HSA二级结构的变化.     

麦塔喇红与蛋白质相互作用的光谱研究

运用紫外光谱法和荧光光谱法研究了有机染料麦塔喇红与牛血清白蛋白(以下简称BSA)的相互作用。 紫外光谱法研究表明,两者之间的结合符合Scatchard模型,存在两类结合,结合数分别为8.4和11.1,结合常数分别为1.1×106 mol-1·L和1.5×105 mol-1·L。 同时通过麦塔喇红与牛血清白蛋白的荧光猝灭对两者的作用机理进行了初步探讨,对蛋白质构象变化进行了分析。     

叶酸与人血清白蛋白结合作用的光谱研究

在不同温度下的pH 7.4的Tris-HCl缓冲溶液体系中, 采用荧光光谱、紫外吸收光谱和同步荧光光谱研究了人血清蛋白与叶酸的相互作用。研究表明,这种相互作用使人血清白蛋白发生内源荧光猝灭,属于静态猝灭机制。通过计算得到人血清蛋白与叶酸在17和37 ℃下静态猝灭的猝灭速率常数分别为7.396 6×104和7.2652×104 L·mol-1、结合常数分别为7.50×104和1.98×105 L·mol-1、结合位点数均为1。根据Förster非辐射能量转移机理,求算出给体(HSA)与受体(叶酸)间的作用距离和能量转移效率分别为1.77和0.052 65 nm,并结合热力学参数说明了叶酸分子与人血清白蛋白的作用以疏水作用为主,同时也存在静电引力。利用同步荧光光谱研究了人血清蛋白与叶酸的相互作用中HSA的构象变化,发现色氨酸残基所处环境的疏水性降低,说明叶酸分子进入了人血清白蛋白的疏水腔中。     

苯酚磺酞类酸性染料与人血清白蛋白的结合

在人体条件下 ,用荧光光谱法研究了苯酚磺酞类酸性染料苯酚红、甲酚红、氯酚红、溴甲酚紫、间甲酚紫与人血清白蛋白 (HSA)之间的相互作用。实验表明 :苯酚磺酞类酸性染料对人血清白蛋白的荧光有较强的猝灭作用 ,其荧光猝灭主要为静态猝灭 ,从荧光猝灭结果求得不同温度下各染料与HSA的结合常数K ,发现染料取代基的引入使K值增大 ,且随反应温度上升K值下降。由染料与HSA反应焓变、熵变 ,确定染料与HSA的结合主要是静电引力。依据非辐射能量转移机理 ,探讨了不同温度下该类染料与HSA相互结合时 ,其给体 受体间距离和能量转移效率。进一步证实了该类反应为单一静态猝灭过程 ,且阐明了其猝灭机理是通过能量转移产生的。     

芦丁钐配合物与血清白蛋白的相互作用

在生理pH值条件下,用荧光光谱法(FS)研究了芦丁钐配合物(rutin-Sm)与牛血清白蛋白(BSA)和人血清白蛋白(HSA)之间的结合反应。探讨了rutin-Sm对BSA 和HSA的荧光猝灭过程的猝灭机理, 以Lineweaver-Burk双倒数方程分别计算了不同温度下rutin-Sm与BSA和HSA的结合常数(K_LB)和热力学参数,并判断rutin-Sm与BSA和HSA结合的作用力类型;实验结果表明:rutin-Sm与BSA和HSA结合形成复合物,导致BSA(HSA)内源性荧光猝灭是由于分子内的非辐射能量转移而引起的静态猝灭;以Lineweaver-Burk方程计算rutin-Sm与HSA和BSA的结合常数KLB分别为:rutin-Sm-HSA, 295 K: 6.830×105 L·mol-1; 310 K: 4.665×105 L·mol-1; rutin-Sm-BSA, 295 K: 6.540×105 L·mol-1; 310 K: 3.265×105 L·mol-1;芦丁钐配合物与BSA之间的作用力主要为范德华力、氢键; 而与HSA之间的作用力主要为静电引力。同时用同步荧光光谱法探讨了rutin-Sm对BSA和HSA构象的影响。进一步证明芦丁钐配合物在体内能够被血清白蛋白存储和转运。     

丹参酮ⅡA等中草药有效成分与白蛋白结合反应的光谱研究

在β－环糊精存在的缓冲体系中,利用光谱法研究了丹参酮ⅡA等有效成分与人血清蛋白(HSA)折结合反应。结果表明：丹参酮ⅡA等与HSA结合后,紫外吸收有红移现象,且吸收强度增加;它们对HSA的荧光有较强的猝灭作用。根据Lineweaver-Burk双倒数图,求得了它们与HSA的解离常数,基于Foerster无辐射能量转移机理,确定了它们的第一结合部位与HSA中214位色氨酸残基的距离。     

光谱法和分子对接模拟技术研究异烟肼对人血清白蛋白和过氧化氢酶的特异性结合及抑制作用

异烟肼(Isoniazid, INH)是最常用的一线抗结核药物之一。据报道,人体内高浓度的异烟肼可导致癫痫, 肝功能衰竭, 甚至死亡。因此,研究异烟肼对人血清白蛋白(HSA)和过氧化氢酶(CAT)的结构和活性的潜在结合影响有利于评估其毒性和副作用。在模拟生理条件下,利用多种荧光光谱和分子对接技术研究INH与HSA和CAT之间的相互作用。所有荧光数据均进行了内滤光校正以获得更准确的结合参数。结果表明,INH-HSA和INH-CAT体系的猝灭常数(K_sv)随着温度的升高而降低,表明INH对HSA及CAT的荧光猝灭机理为静态猝灭。利用紫外-可见吸收光谱、同步荧光光谱、和圆二色(CD)光谱法研究了INH对HSA和CAT构象的影响。结果发现,INH可改变色氨酸残基的微环境并降低HSA和CAT中α-螺旋结构,导致蛋白质结构发生伸展,进而可能影响其生理功能。分子对接结果表明,INH与HSA的结合位点位于HSA的site Ⅰ,ⅡA子域。INH可以进入CAT中β-折叠的桶状空腔,从而抑制CAT的活性。Hill系数结果表明,INH与左氧氟沙星(LVFX,一种安全有效的二线抗结核药物,与其他抗结核药物联合使用可以提高抗结核疗效)之间存在药物协同性,促进INH与HSA的相互作用。另外,CD光谱测定表明INH与LVFX的协同作用改变HSA的二级结构,使α-螺旋结构降低约7.9%。该研究探讨了INH与HSA和CAT之间的结合作用和毒性机制,为INH的安全使用提供重要依据。     

光谱法和分子对接模拟技术研究异烟肼对人血清白蛋白和过氧化氢酶的特异性结合及抑制作用（英文）

异烟肼(Isoniazid,INH)是最常用的一线抗结核药物之一。据报道,人体内高浓度的异烟肼可导致癫痫,肝功能衰竭,甚至死亡。因此,研究异烟肼对人血清白蛋白(HSA)和过氧化氢酶(CAT)的结构和活性的潜在结合影响有利于评估其毒性和副作用。在模拟生理条件下,利用多种荧光光谱和分子对接技术研究INH与HSA和CAT之间的相互作用。所有荧光数据均进行了内滤光校正以获得更准确的结合参数。结果表明,INH-HSA和INH-CAT体系的猝灭常数(Ksv)随着温度的升高而降低,表明INH对HSA及CAT的荧光猝灭机理为静态猝灭。利用紫外-可见吸收光谱、同步荧光光谱、和圆二色(CD)光谱法研究了INH对HSA和CAT构象的影响。结果发现,INH可改变色氨酸残基的微环境并降低HSA和CAT中α-螺旋结构,导致蛋白质结构发生伸展,进而可能影响其生理功能。分子对接结果表明,INH与HSA的结合位点位于HSA的siteⅠ,ⅡA子域。INH可以进入CAT中β-折叠的桶状空腔,从而抑制CAT的活性。Hill系数结果表明,INH与左氧氟沙星(LVFX,一种安全有效的二线抗结核药物,与其他抗结核药物联合使用可以提高抗结核疗效)之间存在药物协同性,促进INH与HSA的相互作用。另外,CD光谱测定表明INH与LVFX的协同作用改变HSA的二级结构,使α-螺旋结构降低约7.9%。该研究探讨了INH与HSA和CAT之间的结合作用和毒性机制,为INH的安全使用提供重要依据。     

秋水仙碱与人血清白蛋白相互作用的谱学研究

采用紫外、荧光和圆二色光谱研究了秋水仙碱与人血清白蛋白之间的相互作用。结果发现秋水仙碱使人血清白蛋白的紫外吸收增强,特征荧光峰猝灭,并且随温度升高猝灭常数K_SV降低。求算了不同温度下秋水仙碱与人血清白蛋白相互作用的平衡常数与结合位点数。根据Van’t Hoff方程计算出ΔH=-11.66 kJ·mol-1,ΔS=51.507 J·(mol·K)-１,得出二者之间的作用力主要是静电作用力。圆二色光谱测得加入秋水仙碱后人血清白蛋白的α-螺旋降低,二级结构改变,表明秋水仙碱对人血清白蛋白的荧光猝灭机制属于形成配合物所引起的静态猝灭。     

山姜素与人血清白蛋白相互作用的荧光光谱法研究

利用荧光光谱法和紫外-可见光谱法研究了山姜素与人血清白蛋白(HSA)之间的相互作用。证实了山姜素对HSA的荧光猝灭为动态猝灭过程,并测定了不同温度下的猝灭常数; 根据Fōrster非辐射能量转移理论,计算出山姜素在蛋白质中的结合位置与色氨酸残基间的距离为4.05 nm; 由求得的热力学参数,推断了山姜素与HSA之间主要靠疏水作用力结合;用三维荧光光谱及同步荧光光谱技术探讨了山姜素对HSA构象的影响。     

三种异黄酮类药物与不同异构体人血清白蛋白的作用机制研究

利用荧光光谱研究了三种异黄酮类化合物染料木素、鸡豆黄素A和3’,4’,7-三羟基异黄酮与不同异构体人血清白蛋白的相互作用机制。计算了异黄酮与蛋白质形成复合物的各种结合参数(猝灭速率常数、结合常数及结合位点数),结果表明三种异黄酮类化合物在人血清白蛋白上只有一个结合位点,位于结合位点siteⅠ,结合常数在0.17×105～1.20×105 L.mol-1之间。荧光增强光谱结果显示,与蛋白质作用后药物的荧光强度明显增加,说明了药物与人血清白蛋白发生了结合,在此基础上讨论了三种异黄酮与人血清白蛋白的结合机理。     

Interaction of human serum albumin with N-(4-ethoxyphenyl)-N′-(4-antipyrinyl) thiourea using spectroscopies and molecular modeling method

The interaction between N-(4-ethoxyphenyl)-N′-(4-antipyrinyl) thiourea (EPAT) and human serum albumin (HSA) was studied by fluorescence spectroscopy in combination with UV absorption spectroscopy. The intrinsic fluorescence of human serum albumin was quenched by EPAT through a static quenching procedure. The binding constants of EPAT with HSA were estimated according to the fluorescence quenching results at different temperatures. The binding distance was obtained and the binding force was suggested to be mainly hydrophobic force, which was in accordance with the study of molecular model. The effect of common ions on the binding constants was also investigated. A new fluorescence spectroscopy assay of the proteins is presented, and results were very satisfactory.     

光谱法研究染料木素与人血清白蛋白的相互作用

用荧光猝灭光谱、同步荧光光谱和紫外-可见吸收光谱研究了染料木素与人血清白蛋白(HSA)的相互作用。结果表明染料木素对HSA的荧光猝灭作用属于二者形成复合物所引起的静态猝灭;利用Stern-Volmer方程处理实验数据,得到染料木素与HSA之间的结合常数K_A为1.00×106(27 ℃),1.66×106(37 ℃)和5.25×106(47 ℃)。根据Frster非辐射能量转移理论,求出了染料木素与HSA之间的结合距离为2.59 nm(27 ℃),2.65 nm(37 ℃)和2.90 nm(47 ℃)。通过计算热力学参数,可知该药物与人血清白蛋白的相互作用是一个吉布斯自由能降低的自发过程,且二者之间的主要作用力类型为静电引力,同时用同步荧光光谱探讨了染料木素对HSA构象的影响。     

Characterization of Interaction Between Bergenin and Human Serum Albumin in Membrane Mimetic Environments

The interaction between bergenin and human serum albumin (HSA) in AOT/isooctane/water microemulsions was studied by fluorescence quenching technique in combination with UV absorption spectroscopy, circular dichroism (CD) spectroscopy and dynamic light scattering (DLS) technique. Fluorescence data in omega (o) 20 microemulsions revealed the presence of a binding site of bergenin on HSA and its binding constants (K) were 1.64 x 10(4), 1.44 x 10(4), 1.26 x 10(4) and 1.09 x 10(4) M(-1) at 289, 296, 303, and 310 K, respectively. The binding of bergenin with HSA in microemulsions was stronger than that in buffer solution. The alterations of protein secondary structure in the microemulsions in the absence and presence of bergenin compared with the free form of HSA in buffer were qualitatively and quantitatively analyzed by the evidence from CD spectra. Enthalpy and entropy changes for the reaction were calculated to be -14.45 kJ mol(-1) and 30.76 J mol(-1) K(-1). These results indicated that bergenin bound to HSA mainly by a hydrophobic interaction in microemulsions which was in agreement with the result of the molecular modeling study. The DLS data suggested that HSA may locate at the interface of the microemulsion and bergenin could interact with them.     

Optical, Structural and Thermodynamic Studies of the Association of an Anti-leucamic Drug Imatinib Mesylate with Transport Protein

The interaction of an anti-leukemic drug, imatinib mesylate (IMT) with human serum albumin (HSA) was investigated by fluorescence, synchronous fluorescence, three-dimensional fluorescence, circular dichroism and UV–vis absorption techniques under physiological condition. The process of binding of IMT on HSA was observed to be through a spontaneous molecular interaction procedure. IMT effectively quenched the intrinsic fluorescence of HSA via static quenching. The values of binding constant, number of molecules that interact simultaneously with the binding site and thermodynamic parameters were evaluated by carrying out the interactions at three different temperatures. Based on thermodynamic parameters and displacement studies with site probes, it was proposed that the drug bound at Sudlow’s site I of subdomain IIA. The change in the conformation of HSA was evident from synchronous, three-dimensional fluorescence and circular dichroism studies. The distance between the donor (protein) and acceptor (drug) was calculated based on the Foster’s theory of resonance energy stransfer and it was found to be 1.30 nm. The effect of different metal ions on the binding of the drug to protein was also investigated.     

The binding of 3-(p-bromophenyl)-5-methyl-thiohydantoin with human serum albumin: Investigation by fluorescence spectroscopy and molecular model

The binding of 3-(p-bromophenyl)-5-methyl-thiohydantoin (BPMT) with human serum albumin (HSA) was investigated by fluorescence spectroscopy in combination with UV absorption spectrum under physiological conditions. The intrinsic fluorescence of HSA was quenched by BPMT through static quenching mechanism and the fluorescence emission spectrum of HSA exhibited appreciable hypsochromic shift with increasing concentration of BPMT. The binding constants (K) of HSA with BPMT and the number binding sites (n) at different temperatures, thermodynamic parameter enthalpy changes (ΔH) and entropy changes (ΔS) of HSA-BPMT have been calculated according to the relevant fluorescence data, indicating that the hydrophobic interaction played a major role, which was consistent with the result of molecular modeling study.     

Study of the Interaction of Fangchinoline with Human Serum Albumin by Fluorescence and UV Spectroscopic Method

The interaction of fangchinoline with human serum albumin (HSA) was studied by use of fluorescence quenching spectra, synchronous fluorescence spectra, and ultraviolet spectra. It was shown that fangchinoline has a strong ability to quench the fluorescence of HSA. The Stern‐Volmer curves based on the quenching of the fluorescence of HSA by fangchinoline indicated that the quenching mechanism of fangchinoline on HSA was static quenching and non‐radiation energy transfer. Based on the Förster theory of non‐radiation energy transfer, the binding distances (r) and the binding constants (K _A) between fangchinoline and HSA were found. The thermodynamic parameters obtained revealed that the interaction between fangchinoline and HSA was mainly driven by hydrophobic force. The conformational changes of HSA were investigated by use of synchronous fluorescence. The result indicates that an ionic electrostatic interaction between fangchinoline and HSA could not be excluded.