甲苯咪唑共振散射法用于蛋白质的痕量检测

建立了血液中痕量蛋白的共振散射(RLS)光谱分析方法。盐酸-甲苯咪唑(MEB)-牛血清白蛋白(BSA)体系的最大共振散射(RLS),二级散射(SOS),倍频散射(FDS)波长分别位于296、500和340nm。3种散射增强(ΔI)在一定范围内与蛋白质浓度成正比,方法线性范围分别是RLS为0.4～2.0 mg/L、SOS为0.4～2.4 mg/L;FDS为0.4～2.0 mg/L;检出限分别为1.059(RLS)、1.324(SOS)、4.743μg/L(FDS)。方法可用于血清中蛋白质的测定,回收率在97.9%～104.6%之间。     

液相色谱-质谱法测定人体血浆中非那雄胺含量

建立了测定人体血浆中非那雄胺药物浓度的液相色谱-质谱分析方法。色谱柱为Hypersil-Keystone C_(18)柱,流动相为乙腈∶水(含0.2%三氯乙酸)=55∶45(V/V),质谱选择电喷雾正离子源(ESI+),选择离子模式(SIM)监测,非那雄胺和内标卡马西平质荷比分别为m/z373和m/z237。血浆样品经乙腈去蛋白、离心和吹干后,残渣用流动相溶解。当非那雄胺的浓度在0.5~120ng·mL~(-1)范围时线性关系良好(r=0.999),检测限(S/N=3)为0.02ng·mL~(-1);日间和日内测定的精密度(RSD)分别在6.4%~2.2%和5.5%~1.7%之间;加标0.5ng·mL~(-1)、40ng·mL~(-1)和80ng·mL~(-1)非那雄胺的平均回收率(n=6)分别为108.5%、101.2%和98.7%。方法快速、准确和灵敏,已成功用于人血浆中非那雄胺浓度的测定和人体药代动力学研究。     

表面活性剂和染料探针共振光散射法测定蛋白质

在pH为2.1的Britton-Robinson缓冲溶液中,蛋白质与十二烷基磺酸钠和吖啶红作用形成聚集体,导致体系产生较大的共振散射光(RLS)强度,并且RLS的增强程度与蛋白质的浓度呈线性关系,据此建立了测定蛋白质含量的方法.人血清白蛋白(HSA)和牛血清白蛋白(BSA)分别在0.03～3.0μg/mL和0.2～7.0μg/mL的浓度范围内与增强的共振光散射强度有良好的线性关系,相应的检测限分别为0.0119μg/mL和0.026μg/mL.对体系的反应机理进行了讨论.将方法用于人血清中蛋白质含量的测定,并将分析结果与考马斯亮蓝法进行了对照.t-检验证明,两种方法无显著性差异.     

共振散射猝灭法测定氯酚类环境雌激素

研究了在pH 2.6的tris-HCl缓冲介质中,氯酚类环境雌激素(CPs-EEs)使木质素桃红(Lignin pink LP)与人血清白蛋白(Human Serum Albumin HSA)作用产生的共振光散射(RLS)峰迅速降低.且RLS猝灭程度与一定浓度范围内的CPs-EEs呈线性关系,据此建立了一种测定CPs-EEs的新方法,线性范围为0.033～2.50 μg/mL,检出限为31.1 ng/mL,联用固相萃取分离技术用于实际水样中CPs-EEs(以PCP计算)的测定,相对标准偏差小于3.4%,样品加标回收率为92.1%～100.9%.     

液相色谱-四级杆飞行时间质谱法检验血液中的3-氯甲卡西酮

本研究建立了液相色谱-四级杆飞行时间质谱(LC-QTOF-MS)检验血样中3-氯甲卡西酮(3-CMC)的方法。血液经1:2体积的乙腈沉淀蛋白后,采用Agilent?ZORBAX Eclipse Plus C18色谱柱(3.0 mm×150 mm,1.8μm)分离,0.1%(v/v)甲酸-水(5mol·L~(-1)乙酸铵)和乙腈作为流动相梯度洗脱,电喷雾双喷离子源电离正离子模式(Dual AJS ESI+)扫描。3-氯甲卡西酮在5～500ng·mL~(-1)范围内线性关系良好,检出限和定量限分别为2ng·mL~(-1)和5ng·mL~(-1),回收率在103.6%～113.7%之间,日内精密度小于8.1%,日间精密度小于11.8%。本方法可以对血液中的3-氯甲卡西酮进行定性定量检测,能够满足实际检案的要求。     

微分脉冲溶出伏安法结合化学计量学测定醚类除草剂

在pH=6.82的Britton-Robinson缓冲溶液中,采用循环伏安法和微分脉冲溶出伏安法对醚类除草剂甲羧除草醚(Bifenox)和三氟羧草醚(Acifluofen)的伏安行为进行了研究,发现吸附时间为50 s时此电化学体系达到平衡,而且微分脉冲溶出伏安法能给出较高的灵敏度,甲羧除草醚和三氟羧草醚分别在-685 mV和-700 mV处具有良好还原峰,但由于峰电位接近而谱峰重叠,很难分别测定.本文采用化学计量学方法来解析重叠峰并完成这两种除草剂的定量分析.甲羧除草醚和三氟羧草醚的测定线性范围分别为0.02～0.18 μg·5mL~(-1)和0.02～0.16 μg·5mL~(-1),检出限分别为0.0073 μg·5mL~(-1)和0.0068 μg·5mL~(-1).利用该方法对水样中的甲羧除草醚和三氟羧草醚进行直接测定,获得了较好的定量分析结果.     

十二烷基苯磺酸钠增敏乙基紫共振光散射法测定人尿中痕量1-羟基芘

基于乙基紫(EV)与1-羟基芘(1-OHP)反应形成离子缔合物,导致体系的共振光散射(RLS)增强,建立了测定1-OHP的共振光散射法.在pH 8.0Tris-HCl缓冲介质中,最大RLS峰位于396 nm,其强度与1-OHP浓度成线性关系.加入表面活性剂十二烷基苯磺酸钠(SDBS),体系的灵敏度可提高两倍以上.方法的线性范围为4.0～982 μg·L-1,相关系数r=0.999 4,检出限1.2 μg·L-1,相对标准偏差为5.8%～7.9%,平均回收率为94%(n=6).已成功用于人尿中痕量1-OHP的测定,结果满意.     

超声-伏安法对饮用水中痕量铅(Ⅱ)和铜(Ⅱ)的检测研究

以金纳米粒子修饰玻碳电极为工作电极,采用超声-微分脉冲阳极溶出伏安法连续测定饮用水中痕量铅(Ⅱ)和铜(Ⅱ).通过原子力显微镜(AFM)对金纳米粒子的形貌和大小进行表征,对超声波提高伏安检测信号的工作机理作了比较详细的探讨.实验结果表明,超声波-伏安法提高了方法的灵敏度,与传统的微分脉冲伏安法相比,Pb(Ⅱ)和Cu(Ⅱ)的峰电流分别增大10倍和8倍.Pb(Ⅱ)和Cu(Ⅱ)离子在质量浓度10～250 μg·L-1和5～200 μg·L-1范围内成良好的线性关系,相关系数分别为0.9943和0.9985.在含有50 μg·L-1 Pb(Ⅱ)和20 μg·L-1 Cu(Ⅱ)的溶液中重复测定9次,其相对标准偏差为3.5%和2.2%,Pb(Ⅱ)和Cu(Ⅱ)的检出限分别为0.3 ng·mL-1和0.1 ng·mL-1.该方法成功应用于饮用水中痕量Pb(Ⅱ)和Cu(Ⅱ)的检测,方法简便可靠,具有实际应用意义.     

丽春红G 用于人血清样品中总蛋白的共振光散射测定

在酸性介质中 ,丽春红G (PonceauG ,PG)与牛血清白蛋白 (BSA)、人血清白蛋白 (HSA)、溶菌酶 (Lys)及γ 球蛋白 (γ IgG)等蛋白质作用产生共振光散射 (RLS)增强信号 ,最大散射峰位于 2 88nm处。在最佳酸度和离子强度下 ,增强RLS强度在 2 88nm处与蛋白质的浓度呈线性关系 ,用于测定BSA、HSA、Lys、γ IgG的检出限均在 2 5 μg L以下。本方法成功地应用于合成样和人血清样品的测定 ,测量结果与考马斯亮蓝法一致     

气相色谱法测定工业废水中挥发酚

提出了工业废水样品中的挥发性酚经预先用溴衍生化后用环己烷萃取分离,分取部分萃取液作气相色谱分析的方法.用此方法测定了苯酚、邻甲酚、间甲酚及对甲酚4种挥发酚,所测得的线性范围分别为0.008～80μg·L-1,0.010～100 μg·L-1,0.018～100 μg·L-1,0.012～100 μg·L-1,检出限(S/N=3)分别为8.4 ng·L-1,10.6 ng·L-1,19 ng·L-1,12.8 ng·L-1,测得其回收率在87%～91%之间,相对标准偏差(n=6)在4.0%～7.0%之间.     

苋菜红—蛋白质体系的共振光散射光谱研究及其分析应用

研究了染色剂苋菜红与蛋白质的结合反应,在ＰＨ３．８７的Ｃｌａｒｋ－Ｌｕｂｓ缓冲介质中,苋菜红与蛋白质通过分子间作用力形成复合物。使最大波长约为３６４ｎｍ的共振光散射光谱得到加强。以苋菜红为标记物根据其共振光散射的增强程度。可用于蛋白质的定量测定,其线性响应范围为０－５．０ｍｇ／Ｌ。方法的稳定性及选择性良好,用于人血清试样中总蛋白的测定,结果与经典的考马斯亮兰法一致。     

Rapid and sensitive determination of proteins by enhanced resonance light scattering spectroscopy of sodium lauroyl glutamate

A rapid and sensitive method for the determination of proteins is proposed based on the measurements of the enhanced resonance light scattering (RLS) spectroscopy of sodium lauroyl glutamate (SLG). Under the optimum conditions, the interaction between SLG and proteins occurred rapidly, resulting in greatly enhanced RLS intensity with the maximum peak located at 394 nm. It was found that the enhanced RLS intensities were in proportion to the concentrations of proteins in the range of 0.01-3.1 μg ml⁻¹ depending on the kind of proteins. The detection limits were below 6 ng ml⁻¹. Compared with some other methods for the determination of proteins, this method shows high sensitivity, low detection limit and simplicity. This is an inexpensive, simple and fast one-step procedure which requires only measuring the RLS intensities. Human serum samples were determined with satisfactory results.     

Microdetermination of proteins with the arsenazo-DBN-Al(III) complex by Rayleigh light-scattering technique and application of the method

The determination of proteins with arsenazo-DBN and Al3+ by Rayleigh light-scattering (RLS) is described. The weak RLS of arsenazo-DBN and BSA can be enhanced greatly by addition of Al3+ in the pH range 5.3-7.0; this resulted in two enhanced RLS signals at 420-440 nm and 460-480 nm. The reaction between arsenazo-DBN, Al3+, and proteins was studied and a new method was developed for quantitative determination of proteins. This method is very sensitive (0.34-41.71 microg mL(-1) for bovine serum albumin, BSA, and 0.29-53.41 microg mL(-1) for human serum albumin, HSA), rapid (< 2 min), simple (one step), and tolerant of most interfering substances. The effects of different surfactants were also examined. When these proteins were determined in four human serum samples the maximum relative error was not more than 2% and the recovery was between 97 and 103%.     

Determination of protein by its enhancement effect on the Rayleigh light scattering of carboxyarsenazo

This is the first report on the determination of proteins based on the interaction with carboxyarsenazo (CAA) by Rayleigh light scattering (RLS). At pH 4, the weak RLS of CAA can be enhanced greatly by the addition of proteins, resulting in three characteristic peaks. Based on this, the interactions of CAA with nine kinds of proteins were studied and a new quantitative determination method for proteins has been developed. This method is very sensitive (0.10-15.3 mug ml(-1) for bovine serum albumin (BSA)), rapid (<2 min), simple (one step), tolerant of most interfering substances, and gives a close value to that of the Coomassie brilliant blue (CBB) method in the determination of proteins in human serum. Thus, the CAA assay can be useful for routine analytical purposes and may overcome some of the limitations of other currently employed methods. Mechanism studies show that the three RLS peaks correspond to the absorption valleys of the CAA-protein complex.     

A resonance light-scattering determination of proteins with fast green FCF.

The interaction of Fast Green FCF (FCF) with proteins (including bovine serum albumin (BSA), human serum albumin (HSA), pepsin (Pep) and alpha-chymotrypsin (Chy), and lysozyme (Lys)) was characterized by enhanced resonance light-scattering (RLS) measurements using a common spectrofluorometer. The enhanced RLS signals of FCF by proteins at 279.0 nm were obtained, and the mechanism of the RLS enhancement was considered in terms of the effects of the pH and ionic strength on the interaction. It was found that the enhanced RLS intensities were in proportion to the concentrations of proteins in the range of nanogram levels, displaying that the present assay is much more sensitive than the reported RLS methods, with the limits of determination being 4.54, 0.6, 22.8, 4.32 and 1.75 ng/ml for BSA, HSA, Pep, Chy, and Lys. respectively.     

Study of the reaction of proteins with Beryllon II-AlIII by the Rayleigh light scattering technique and its application

The determination of proteins with tetrasodium 2-(3,6-disulfo-8-hydroxynaphthylazo)-1,8-dihydroxynaphthalene-3,6-disulfonate (Beryllon II) by Rayleigh light scattering (RLS) was studied. The weak RLS of the Beryllon II-bovine serum albumin (BSA) complex can be greatly enhanced by the addition of Al3+ in the pH range 5.6-7.2; there was a maximum RLS platform at 400-420 nm. Based on the reaction between Beryllon II, Al3+ and proteins, a new method for the determination of proteins was developed. This method is very sensitive [0.20-41.42 micrograms ml-1 for BSA and 0.18-48.15 micrograms ml-1 for human serum albumen (HSA)], rapid (< 2 min), simple (one step) and tolerant towards most interfering substances. The effects of different surfactants were also examined. Four samples of protein in human serum were determined; the maximum relative error was no more than 5% and the recovery was 96-105%.     

Determination of proteins at nanogram levels based on their enhancement effects of Rayleigh light scattering on dibromomethylchlorophosphonazo

A new Rayleigh light scattering (RLS) assay of protein was conducted in this paper. At the optimum pH conditions, and in the presence of Tween-20, the weak RLS of dibromomethylchlorophosphonazo (DBM-CPA) can be enhanced greatly by the addition of proteins. Based on this, the reactions of DBM-CPA and proteins were studied. A new quantitative determination method for proteins has been developed. The method is simple, practical and relatively free from interference from coexisting substances, as well as much more sensitive (the dynamic ranges of 0.065-40.05 microg ml(-1) and detection limit of 30 ng ml(-1) for bovine serum albumin (BSA)) than most of the existing assays. The determination results of human body serum samples are identical to those by the CBB method, with relative S.D. of six determination of 0.5-2.2%.     

Resonance Light Scattering Method for Microdetermination of Proteins Based on Aggregation of Au Nanoparticles

By using a resonance light scattering (RLS) technique, a highly sensitive method for protein determination based on the aggregation of Au nanoparticles on protein template is described. For the Au nanoparticles of 15 nm, the detection limit of bovine serum albumin was 5.0 ng/mL and the linear range was 10–300 ng/mL. The experimental results indicated that various metal ions do not interfere with this assay. The proposed RLS assay exhibited lower variation in response signals for the same weight of different proteins and showed satisfactory results when it was used for determination of proteins in human serum.     

A Novel Protein Assay With an Azo Dye Using Rayleigh Light Scattering Technioque

ABSTRACT

The interaction of SPADNS [3-(4-sulfophenylazo)-4, 5-dihydroxy-2, 7-naphthalene disulfonic acid] with proteins in acidic solution was studied by spectrophotometric and Rayleigh light scattering (RLS) methods. SPADNS reacts rapidly with albumin at room temperature, and the intensity of the weak RLS of SPADNS was enhanced remarkably and quantitatively by this reaction.

Based on this observation, a novel RLS method for serum albumin determination was developed. The linear range is 0.125-14.9 μg/ml for BSA. The relative standard deviation (n=10) for 5.0 μg/ml BSA was 3.94%. The method was applied to the determination of proteins in human plasma, and the results were compared with the traditional proteins assay (CBB method). There is almost no interference from amino acids, metal ions and other coexistent substances. The reaction mechanism was also discussed.     

A Study on the Reaction of Protein with Arsenazo III by Rayleigh Light Scattering Technique

Abstract

A new rayleigh light scattering (RLS) assay of protein was conducted in this paper. The weak RLS of arsenazo III can be enhanced greatly by the addition of proteins. Based on this, the reaction of arsenazo III and proteins was studied. A new quantitative determination method for proteins has been developed. This method is very sensitive (0.085(021.25 μg/mL for BSA), rapid (<1min), simple (one step) and free of interference from most diverse substances.