碱性介质中茜素黄R与牛血清蛋白相互作用研究

在碱性条件下,采用紫外—可见分光光度法研究了茜素黄R(Alizarin Yellow R)与牛血清白蛋白(BSA)的结合反应。研究表明,AYR—BSA二元配合物的最大吸收波长为386 nm,比AYR紫移约108 nm;建立了碱性条件下以AYR测定蛋白质的光谱分析法,对样品分析表明,回收率为96.4%~106.6%,相对标准偏差为0.28%~1.13%;采用双波长法、平衡透析法和单波长法对AYR与BSA的相互作用的研究结果基本一致,在386 nm处,AYR—BSA配合物的结合比为nAYR:nBSA=5 1,摩尔吸光系数ε=9.12×103L.mol-1.cm-1,相互作用的条件平衡常数K=8.13×105。     

Human Serum Albumin Hybrid Incorporating Synthetic Hemes:A Novel O_2-Carrying Hemoprotein

It has long been known that homologous blood transfusion will result in a lot ofserious problems such as viral infections,for example AIDS,hepatitis,antigenicsensitization and GVHD;therefore aggressive testing of donor blood has beenadopted[1 ,2 ] .Even after this introduction,which is time-consuming and expensive,wecould not eliminate all the risks. In the wake of these kinds of pitfalls,production andclinical use of the blood substitutes have emerged.The essential aim of blood substitutei…     

CE determination of quinolones in the presence of bovine serum albumin

This article describes the influence of bovine serum albumin (BSA) as an additive on the capillary electrophoresis–potential gradient determination of five quinolones, enoxacin, norfloxacin, ofloxacin, fleroxacin, and pazufloxacin. With 10 mg/L of BSA present in the buffer of 30 mM Tris and 3 mM phosphoric acid at pH 9, the detection limits of the five quinolones were in the range of 0.24–0.68 mg/L, i. e. 5.8–16.5‐fold lower than those obtained with the buffer devoid of BSA, and the analysis time was shortened. We suggest that the inner wall‐adsorbed BSA suppresses the adsorption of quinolones and simultaneously enhances the electroosmotic flow rate. Our experiments indicated that adopting the potential gradient detection technique could eliminate the interference of the UV‐active proteins on the detection of quinolones that would occur with conventional optical detection, and therefore offer high detection sensitivity. As a demonstration, the method was applied to the determination of QNs in fortified chicken muscle sample with satisfactory results.     

Molecular simulation of the interaction between novel type rhodanine derivative probe and bovine serum albumin

The interaction between 3-(4′-methylphenyl)-5-(4′-methyl-2′-sulfophenylazo) rhodanine (M4MRASP) and bovine serum albumin (BSA) was studied by using spectrofluorimetry. It was shown in fluorescence spectrums that the quenching mechanism of BSA by M4MRASP was a static quenching. Meanwhile, the binding constant and binding site numbers were calculated. The action distance (r = 8.03 nm) and energy transfer efficiency (E = 0.12) between donor (BSA) and acceptor (M4MRASP) were obtained according to the theory of Förster non-radiation energy transfer. The effect of M4MRASP on the conformation of BSA was further analyzed by using synchronous fluorescence spectrometry. A new model of the interaction between small organic molecule and biomacromolecule was established. The results offered a reference for the studies on the biological effects and action mechanism of small molecule with protein.     

利用发光细菌测定人体血清杀菌活性的研究

本文报导了以发光细菌作指示生物,以相对发光强度的变化为指标,测定人体血清样品总补体活性(CH_(50))的新方法。当把发光细菌和正常人体血清混和培养时,由于血清的杀菌作用而使细菌体内发光强度减弱,且光强度的减弱程度直接与活菌数的减少以及血清浓度相关联。用这一方法测定了199个人体血清样品,并与常规方法测定结果作比较,表明所有CH_(50)值正常的人血清样品抑制细菌发光能力明显大于CH_(50)值不正常的人血清样品,而且抑制细菌发光50％所得结果与常规CH_(50)试验结果一致。发光细菌测定法是一种简便、快速、灵敏的方法。     

The electrochemical behavior of N-n-undecyl-N''-(sodium-p-amino-benzenesulfonate)thiourea and its interaction with bovine serum albumin

In pH 5.5 phosphate buffer solution,N-n-undecyl-N'-(sodium-p-amino-benzenesulfonate)thiourea(UPT)produced a pair of redox peaks on the bare glassy carbon electrode.At the multi-walled carbon nanotube(MWNT)modified electrode,the electrochemical behavior of UPT enhanced greatly.In the presence of bovine serum albumin (BSA),the peak currents of UPT decreased linearly due to the formation of a super-molecular complex.This method was successfully applied to the determination of BSA in a bovine serum sample.     

氨基硅球表面印迹牛血清白蛋白分离条件的初步探讨

采用固定模板蛋白表面印迹的方法,在氨丙基衍生的硅球表面制备溶胶-凝胶印迹聚合物识别牛血清白蛋白.以该体系为例对制备蛋白质印迹聚合物的各个基本参数与分离选择性的关系进行研究.结果表明,用正辛基三甲氧基硅烷、氨丙基三乙氧基硅烷、四乙氧基硅烷在摩尔比为42.5:42.5:15,酸度为pH 7.0时进行聚合,并采用01 mol/L NaOH与10%(V/V) HAc-10%(m/V) SDS联用的方法洗脱固定的模板蛋白,由此制备的印迹聚合物的分离选择性能较好;并初步讨论了识别蛋白质的机理.     

Determination of glibenclamide in human serum by HPLC

The antidiabetic drug glibenclamide can be reliably quantitated in human serum with high performance liquid chromatography. The serum is buffered and extracted with toluene. The organic solvent is evaporated, the residue dissolved in the mobile phase and an aliquot sampled automatically and chromatographed. UV-detection at 229 m allows a lower limit of quantitation of 5 ng/ml. Precise handling of exact volumes facilitates external calibration. Statistical data for imprecision and inaccuracy are given and illustrate reliable quantification. Application of the method to experimental and clinical pharmacokinetic studies with specific problems is illustrated.     

On‐line 2D‐LC‐ESI/MS/MS determination of rifaximin in rat serum

A highly sensitive and selective on‐line two‐dimensional reversed‐phase liquid chromatography/electrospray ionization–tandem mass spectrometry (2D‐LC‐ESI/MS/MS) method was developed and validated to determine rifaximin in rat serum by direct injection. The 2D‐LC‐ESI/MS/MS system consisted of a restricted access media column for trapping proteins as the first dimension and a Waters C₁₈ column as second dimension using 0.1% aqueous acetic acid:acetonitrile as mobile phase in a gradient elution mode. Rifampacin was used as an internal standard. The linear dynamic range was 0.5–10 ng/mL (r² > 0.998). Acceptable precision and accuracy were obtained over the calibration range. The assay was successfully used in analysis of rat serum to support pharmacokinetic studies. Copyright © 2009 John Wiley & Sons, Ltd.