Investigation on the binding site in heparin by spectrophotometry

Heparin has a variety of biological activities, most of them due to heparin’s high sulfate groups. To gain insight into the mechanism of activation of the spectroscopic probe with sulfate groups of heparin in vitro, we have used a cationic dye by a spectrophotometric method. It is considered that the combination of heparin with methylene blue is due to noncovalent binding forces. Dye binding requires an organic chain structure form with sulfate groups. The solution equilibria of the reaction system are discussed. A new linear regression equation has been proposed, in which the maximum binding number N expresses the binding ability of methylene blue (MB) with sulfate groups of heparin. The linear regression equation can estimate this parameter.     

Study on the interaction between oxolinic acid aggregates and protein and its analytical application

It was found that oxolinic acid (OA) at high concentration can self-assemble into nano- to micro- meter scale OA aggregates in Tris-HCl (pH 7.48) buffer solution. The nanoparticles of OA were adopted as fluorescence probes in the quantitative analysis of proteins. Under optimum conditions, the fluorescence quenching extent of nanometer scale OA aggregates was in proportion to the concentration of albumins in the range of 3.0 × 10⁻⁸ to 3.0 × 10⁻⁵ g mL⁻¹ for bovine serum albumin (BSA) and 8.0 × 10⁻⁸ to 8.0 × 10⁻⁶ g mL⁻¹ for human serum albumin (HSA). The detection limits (S/N = 3) were 3.4 × 10⁻⁹ g mL⁻¹ for BSA, and 2.6 × 10⁻⁸ g mL⁻¹ for HSA, respectively. Samples were satisfactorily determined. The interaction mechanism of the system was studied using fluorescence, UV-vis, resonance light scattering (RLS) and transmission electron microscope (TEM) technology, etc., indicating that the nonluminescent complex was formed between serum albumin molecular and OA, to disaggregate the self-association of OA, which resulted in the dominated static fluorescence quenching in the system.     

叶酸的平行催化波及其分析应用

在Britton-Robinson(pH 4.1)的缓冲溶液中叶酸于-0.56 V(vs.SCE)产生一还原波,该波能被氧化剂过硫酸钾催化形成平行催化波.催化波峰电位不变,峰电流增加10倍,二阶导数波波高与叶酸的浓度在5.0×10-9～3.5×10-7 mol/L范围内呈线性关系(r=0.999),检出限可达3.0×10-9mol/L.方法简便灵敏,运用该法测定了叶酸片剂中的叶酸.     

Analysis of the disaccharides derived from hyaluronic acid and chondroitin sulfate by capillary electrophoresis with sample stacking

CE conditions for monitoring the unsaturated disaccharides of hyaluronic acid (di-HA) and chondroitin sulfate (di-CS) using an alkaline tetraborate buffer, electrokinetic sample injection, and UV absorption detection at 232 nm are reported. Separations were performed in an uncoated fused-silica capillary having reversed polarity and reversed electroosmosis generated with the addition of CTAB to the buffer. The influence of various separation parameters, including the concentration of CTAB, buffer pH, concentration of tetraborate, and applied voltage, on the resolution of the two disaccharides was investigated. Baseline separation was obtained with 25 mM tetraborate at pH 10.0 and having 0.05 mM CTAB. Chloride and phosphate in the sample are beneficial for the stacking of the disaccharides, with di-HA forming a much sharper peak than di-CS. Using samples prepared in 25 mM Tris-HCl (pH 7.5) and electrokinetic injection at the cathode at -10 kV for 40 s, linear relationships between the corrected peak area and the concentration of the disaccharides have been found in the ranges of 1.0-400.0 and 0.1-1.0 microg/mL (0.2-1.0 microg/mL for di-CS), with correlation coefficients being >0.9933 in all cases. The RSDs of detection times and corrected peak areas were between 1.13-1.24 and 1.57-2.13%, respectively. Applied to human serum samples that were prepared by ethanol precipitation and depolymerization of the two polysaccharides with chondroitinase ABC reveals comigration of endogenous compounds with di-HA and a sample-dependent detection time. The di-HA content in the serum sample can be estimated via subtraction of the blank peak that is obtained without enzymatic hydrolysis.     

尿酸与四氯苯醌的荷移反应及其分析应用

采用紫外分光光度法研究了尿酸与四氯苯醌之间的荷移反应。在乙腈溶液中,尿酸与四氯苯醌可迅速形成稳定的1∶1荷移配合物。其最大吸收波长为450 nm,表观摩尔吸光系数ε=1.52×104L.mol-1.cm-1,线性范围是1.01×10-6~10.1×10-6mol/L。用本法测定人体代谢物中的尿酸,回收率为99.8%~105.6%,相对标准偏差(RSD)为3.48%(n=5)。     

Multi-spectroscopic method study the interaction of anti-inflammatory drug ketoprofen and calf thymus DNA and its analytical application

Interactions of the anti-inflammatory drug ketoprofen with calf thymus DNA (ctDNA) in aqueous solution have been studied by multi-spectroscopic method including resonance light scattering (RLS) technique, ultraviolet spectra (UV), (1)H NMR, etc. The characteristics of RLS spectra, the effective factors and optimum conditions of the reaction have been unequivocally investigated. Mechanism investigations have shown that ketoprofen can bind to ctDNA by groove binding and form large particles, which resulted in the enhancement of RLS intensity. In Critic acid-Na(2)HPO(4) buffer (pH=6.5), ketoprofen has a maximum peak 451.5 nm and the RLS intensity is remarkably enhanced by trace amount of ctDNA due to the interaction between ketoprofen and ctDNA. The enhancement of RLS signal is directly proportional to the concentration of ctDNA in the range of 1.20×10(-6)-1.0×10(-5) mol/L, and its detection limit (3σ) is 1.33×10(-9) mol/L. The method is simple, rapid, practical and relatively free from interference generated by coexisting substance, and was applied to the determination of trace amounts of nucleic acid in synthetic samples with satisfactory results.     

A spectroscopic study of the interaction of octacarboxylic metal phthalocyanine with bovine serum albumin

The interaction of octacarboxylic metal phthalocyanines (MPc(COOH)₈, M =?Al(III) and Co(II) with bovine serum albumin (BSA) has been studied. From the binding isotherm based on spectrophotometric titration, the association constant and a number of ligands per binding site were calculated at 25°C. By using the well studied Hemin chloride (HE), Ibuprofen(IB) and L-tryptophan (TRP) as competitive ligands, the binding sites of AlPc(COOH)₈ were found to be on domain I and II of BSA, while on domain I for Co(COOH)₈.     

Synthesis of a novel fluorescent probe and investigation on its interaction with nucleic acid and analytical application

A novel fluorescent probe N-(N-(2-(4-morpholinyl)ethyl)-4-acridinecarboxamide)-alpha-alanine (N-(N-(ME)-4-ACA)-alpha-ALA) was synthesized. The structure was characterized by 1H NMR, MS, elemental analysis, fluorescent and ultraviolet spectra. This new compound exhibited high binding affinity to DNA, intense fluorescence and high water solubility. Experiment indicated that the fluorescent intensity was quenched when DNA was added. A method for DNA determination based on the quenching fluorescence (lambda(ex)=258nm, lambda(em)=451nm) of N-(N-(ME)-4-ACA)-alpha-ALA was established. Under optimal conditions (pH 7.2, CN-(N-(ME)-4-ACA)-alpha-ALA)=3 x 10(-6) mol L(-1)), the linear range is 0.1-4.0 microg mL(-1) for both fish semen (fsDNA) and calf thymus DNA (ct-DNA). The corresponding determination limits are 4.6 ng mL(-1) for fsDNA and 5.1 ng mL(-1) for ct-DNA, respectively. The relative standard deviation is 1.0%. Thus this compound can be used as a DNA fluorescent probe. The experiments proved that the interaction mode between N-(N-(ME)-4-ACA)-alpha-ALA and DNA was groove binding. The modified Rosenthal's graphical method gave the binding constant of 1.0 x 10(6) L mol(-1) and a binding size of 0.31 base pairs per bound drug molecule.     

Studies on the interaction of protein with acid chrome blue K by electrochemical method and its analytical application

An electrochemical investigation on the interaction of acid chrome blue K (ACBK) with protein on the mercury electrode with different electrochemical methods such as cyclic voltammetry and linear sweep voltammetry was reported in this paper. In pH 3.0 Britton-Robinson (B-R) buffer solution, ACBK has an irreversible voltammetric reductive peak at -0.23 V (vs. SCE). The addition of human serum albumin (HSA) into the ACBK solution resulted in the decrease of reductive peak currents without the change of the peak potential and no new peaks appeared on the cyclic voltammogram. In the absence and presence of HSA, the electrochemical parameters such as the formal potential E0, the electrode reaction standard rate constant k(s) and the charge transfer coefficient alpha of the interaction system were calculated and the results showed that there were no significant changes between each other. Thus, the interaction of ACBK with protein forms an electro-inactive supramolecular bio-complex, which induces the decrease of the free concentration of ACBK in the reaction solution, and the decrease of the reductive peak current of ACBK. The binding constant and the binding ratio are calculated as 1.29 x 10(8) and 1:2, respectively, and the interaction mechanism is discussed. Based on the binding reaction, this new electrochemical method is further applied to the determination of HSA with the linear range from 3.0-20.0 mg/L and the linear regression equation as deltaIp"(nA) = 10.08 + 19.90 C (mg/L). This method was further applied to determinate the content of protein in the healthy human serum samples with the results in good agreement with the traditional Coomassie brilliant blue G-250 spectrophotometric method.     

3-羟基邻苯二甲酰亚胺全水溶性次氯酸荧光探针及其应用

利用二甲基硫代氨基甲酸酯对次氯酸(HOCl)的特异性和吡啶盐的水溶性,以4-羟基异苯并呋喃-1,3-二酮作为原料,设计合成了一种检测HOCl的全水溶性激发态分子内质子转移(ESIPT)荧光探针.由于二甲氨基硫代甲酸酯对羟基的保护,探针分子内的ESIPT作用被阻碍,自身无荧光;当加入HOCl时,HOCl氧化二甲氨基硫代甲...     

Study of the interaction of proteins with curcumin and SDS and its analytical application

It is found that protein and sodium dodecyl sulphonate (SDS) can enhance resonance light scattering (RLS) of curcumin (CU). Based on this phenomenon, a new quantitative method for protein in aqueous solution has been developed. In the BR (pH 3.5) buffer, the RLS intensity of CU-SDS system is greatly enhanced by protein. The enhanced RLS is proportional to the concentration of protein in the range of 0.00020-20.0 microgml(-1) for bovine serum albumin (BSA) and 0.00040-1.0 microgml(-1) for human serum albumin (HSA) and their detection limits are 0.16 and 0.041 ngml(-1), respectively. An actual sample is satisfactorily determined. In addition, the interaction mechanism between protein and CU-SDS is also studied by using multi-techniques such as RLS, absorption spectroscopy and fluorescence, zeta potential assay measurement.     

磷酸苯丙哌林与曙红B的相互作用及其分析应用

在pH为3.35的HAc-NaAc酸性介质中,曙红B(EB)与磷酸苯丙哌林(BPP)借助静电作用和疏水作用力发生相互作用形成EB-BPP离子缔合物,导致体系共振光散射(RLS)强度显著增强,并在364 nm处出现最大散射峰。研究了体系的共振光散射光谱,吸收光谱及荧光光谱的特征,考察了实验条件及共存物质的影响。结果表明,在最佳的实验条件下,体系共振散射增强的强度与BPP的浓度在一定范围内呈良好的线性关系,其线性范围为0.04μg.mL-1~2.00μg.mL-1,检出限为14.31 ng.mL-1。据此,建立了一种高灵敏的定量测定活性组分BPP的方法。方法成功地用于药物、血清及尿样中BPP含量的测定。     

Voltammetric studies on the interaction of amikacin with methyl blue and its analytical application

A new method to determine the concentration of amikacin(AMK)using methyl blue(MB)as electrochemical probe was developed in this paper.In pH 4.5 Britton-Robinson(B-R)buffer solution,the MB reacted with AMK to form ion association complexes,which led to the reductive peak current of MB at-0.275 V(versus SCE)to decrease,and the decreases were linear with the concentration of AMK in the range of 1.0-60.0 mg/L,the regression of equation isΔIp(nA)=-8.48 102.36c(mg/L), correlation coefficientγis 0.997.The conditions for determining the concentration of AMK using linear sweep voltammetry(SLV) were optimized.The method was used to determine the content of amikacin commercially available with satisfactory results.     

Electrochemical studies on the interaction of heparin with crystal violet and its analytical application

In this paper, crystal violet (CV) was used to determine heparin concentration by linear sweep voltammetry on a dropping mercury electrode (DME). In Britton-Robinson (B-R) buffer solution, pH 3.0, CV had a well-defined second-order derivative linear sweep voltammetric reductive wave at −0.74 V (vs. SCE). After the addition of heparin to the CV solution, the reductive peak current decreased greatly with the positive movement of the peak potential and without appearance of new peaks in the scanning potential range. Based on the decrease in the reductive peak current, a new voltammetric method for the determination of heparin was established. The conditions for the interaction and the electrochemical detection were optimized, and interfering substances were investigated. Under the optimal conditions, the decrease in reductive peak currents of CV was proportional to heparin concentration in the range 0.1–8.0 mg/L with the linear regression equation Δip″(nA) = 400.42 + 1563.11c (mg/L), (n = 14, γ = 0.993). The detection limit was 0.092 mg/L. This new method was further successfully applied to the determination of heparin content in heparin sodium injection samples with satisfactory results. The binding ratio and binding mechanism were also studied by the electrochemical method. The text was submitted by the authors in English.     

锌试剂与壳聚糖的结合反应机理的研究

为从分子水平认识多糖分子与小分子之间相互作用的机理,应用光谱法研究了壳聚糖(CTS)与锌试剂(ZCN)的相互作用机理;测得ZCN-CTS复合物吸收光谱出现新的吸收峰所需的临界ZCN/CTS摩尔比为2.67×103, CTS对ZCN的最大结合数为6.93×103,实验值与理论值相吻合,证明了多糖与生物探针相互作用理论模型的可靠性;探讨了ZCN与CTS相互作用产生变色反应的机理,认为其是在ZCN与CTS大分子间发生静电相互作用的基础上,主要由ZCN与CTS大分子间的疏水相互作用所引起.     

Fluorometric study of the inclusion interaction of beta-cyclodextrin derivatives with tetraphenylporphyrin and its analytical application

The effects of native beta-cyclodextrin (beta-CD) and four kinds of alkylated beta-cyclodextrin (beta-CDs), i.e. heptakis (2,6-di-O-isobutyl-beta-cyclodextrin) (I), heptakis (2,6-di-O-octyl-beta-cyclodextrin) (II), heptakis (2,6-di-O-dodecyl-beta-cyclodextrin) (III), and heptakis (2,6-di-O-hexadecyl-beta-cyclodextrin) (IV), on the fluorescence behaviors of tetraphenylporphyrin (TPP) are investigated. An obvious fluorescence enhancement is observed from TPP by using alkylated derivatives compared to that obtained in beta-CD aqueous or in water. A 114-N fluorescence emission intensity enhancement is found for the complex with 2,6-di-O-octyl-beta-cyclodextrin relative to the free analyte. The exact stoichiometric ratios and the formation constants of the inclusion complexes have been examined by application of curve fitting method. The linear calibration plots between fluorescence intensity and TPP concentration are determined in the 1.14 x 10(-8)-5.06 x 10(-6) mol l(-1) range.     

Voltammetric study on the interaction of heparin with toluidine blue, and its analytical application

The interaction of heparin with toluidine blue (TB) was studied by voltammetry. In pH 5.8 Britton-Robinson (BR) buffer, heparin, which is negatively charged, easily binds to the positively charged TB to form a polyelectrolyte complex. Due to the formation of the complex, the well-defined redox peaks of TB at the glass carbon electrode decreased correspondingly without the movement of the peak potential after the addition of heparin. The reaction conditions were optimized carefully. Based on the decrease of the peak current of TB solution, a new electrochemical analytical method was established for heparin with a linear range from 1.0 to 20.0 μg mL⁻¹ and a detection limit of 0.44 μg mL⁻¹. The relative standard deviation (RSD) for five parallel determinations of 10.0 μg mL⁻¹ heparin was 1.07%. This new method was applied to the determination of heparin in heparin sodium injection samples with satisfactory results.     

荧光素染料与富马酸酮替芬的光谱研究及应用

在弱酸性缓冲介质中,富马酸酮替芬和某些卤代荧光素类染料(曙红Y、荧光桃红和曙红B)借助静电引力和疏水作用力形成离子缔合物,引起共振光散射光谱、吸收光谱及荧光光谱的变化。实验表明,曙红Y体系灵敏度最高。对曙红Y、荧光桃红和曙红B体系,线性范围分别为0.12~8.4μg/mL、0.24~8.4μg/mL和0.18~6.0μg/mL,检测限分别为12.72 ng/mL、12.52μg/mL和18.21μg/mL。方法已用于分析富马酸酮替芬片剂、血清及尿样。     

Characterization of the interaction between 8-bromoadenosine with human serum albumin and its analytical application

This study was designed to examine the interaction of 8-bromoadenosine with human serum albumin (HSA) by fluorescence spectroscopy in combination with molecular modeling under simulative physiological conditions. The results of fluorescence measurements indicate that 8-bromoadenosine has a strong ability to quench the intrinsic fluorescence of HSA through static quenching procedure. The binding constants (K) at different temperatures and thermodynamic parameters, enthalpy changes (ΔH) and entropy changes (ΔS) were calculated according to the fluorescence data. The results showed that the hydrophobic force played the major role in the binding of 8-bromoadenosine to HSA. The fluorescence experimental results were in agreement with the results obtained by molecular modeling study. The effects of some normal positive and negative ions on the binding constants were also discussed. Moreover, the synchronous fluorescence technique was used to characterize the interaction of 8-bromoadenosine to HSA and successfully applied to determine the total proteins in human serum, urine and saliva samples at room temperature under the optimum conditions with a wide linear range and satisfactory results.     

Development of a BODIPY-based ratiometric fluorescent probe for hypochlorous acid and its application in living cells

A BODIPY-based ratiometric fluorescent probe for HOCl has been designed based on the transduction of thioether to sulfoxide function. This probe features a marked absorption and emission blue-shift upon the HOCl-promoted rapid transduction, enabling the highly selective and ratiometric detection. In addition, the probe works excellently within a wide pH range of 4–10, addressing the existing pH dependency issue. Living cells studies demonstrate that the probe is cell membrane permeable and can be employed successfully to image endogenous HOCl generation in macrophage cells.