电化学发光分析法测定氨基硫脲

基于在碱性介质中,氨基硫脲对罗丹明B的电化学发光具有抑制作用,建立了测定氨基硫脲的电化学发光新方法。运用阶跃脉冲电解方式,在最佳实验条件下,相对电化学发光强度与氨基硫脲的浓度在1.0×10-10～1.0×10-6mol/L范围内呈线性关系,检出限为8.0×10-11mol/L,该法可应用于水样中氨基硫脲含量的测定。     

毛细管电泳电化学发光法分离检测西咪替丁

建立了以三联吡啶钌为发光体系的毛细管电泳电化学发光(CE-ECL)检测系统,并应用于分离和测定西咪替丁片剂中西咪替丁的含量。考察了检测电位,三联吡啶钌(Ru(bpy)32+)的溶液浓度,缓冲液的pH和溶液浓度,分离电压、进样电压与进样时间等因素对分离检测的影响。结果表明:在检测电位1.18V,Ru(bpy)32+溶液浓度为5 mmol/L,磷酸盐缓冲液(PBS)25 mmol/L(pH 7.8),进样时间10 s,进样电位10 kV,运行电位15 kV下,测得西咪替丁线性范围为2.8×10-6~4.0×10-4mol/L,检出限为1.2×10-7mol/L(S/N=3)。对1.0×10-5mol/L的西咪替丁标准溶液连续测定5次,电化学发光强度和迁移时间的RSD分别为3.9%和1.5%。方法已应用于西咪替丁片剂中西咪替丁含量的测定。     

Silica sol/Nano-Au/PVA/L-cysteine修饰金电极电致化学发光测定甲氧氯普胺的研究

在甲氧氯普胺对联吡啶钌具有较好电化学发光增敏效果的基础上,制备出Silica sol/Nano-Au/PVA/L-cysteine修饰金电极,并通过电致化学发光法,考察了联吡啶钌及联吡啶钌-甲氧氯普胺体系在此电极上的电化学及电化学发光行为。该修饰电极对联吡啶钌-甲氧氯普胺体系有良好的电致化学发光响应特性;在最优条件下,在1.0×10-7~1.0×10-4mol/L范围内甲氧氯普胺浓度与其对应的电化学发光强度值线性关系良好,检出限(S/N=3)为1.40×10-9mol/L;通过平行测定1.0×10-5mol/L甲氧氯普胺溶液8次,发光强度值相对偏差(RSD)为1.8%,样品回收率在98.3%~104.4%之间,RSD为2.3%(n=5)。     

电化学发光传感器用于双酚A的检测

利用反相微乳液法制备了Ru(bpy)2+3-SiO2复合纳米粒子(RuSiO2NPs),采用Nafion/多壁碳纳米管(MWCNTs)复合膜技术,实现了对RuSiO2NPs有效而稳定的固定,从而制备了电化学发光传感器,在0.1mol/L磷酸盐缓冲溶液(PBS,pH=7.4,含50mmol/L三正丙胺)介质中,实现了对双酚A(BPA)的免标记检测。在优化实验条件下,电化学发光强度减少值与BPA浓度的负对数在1.0×10-11~1.0×10-7 mol/L范围内呈良好的线性关系,相关系数R=0.9978,检出限为8.0×10-12 mol/L。对1.0×10-9 mol/L BPA平行测定11次,其相对标准偏差为2.7%。实验结果表明该传感器具有良好的稳定性和重现性。     

硅溶胶/Nano-Au固定联吡啶钌电化学发光行为的研究

研究了舒必利在硅溶胶/纳米金/联吡啶钌修饰的金电极上的电化学发光行为,建立了电化学发光法检测舒必利的新方法。在最佳实验条件下,舒必利浓度在1.0×10-6～1.0×10-4mol/L范围内与发光强度呈良好的线性关系(r2=0.9954),检出限(S/N=3)为3.4×10-9mol/L。连续平行测定1.0×10-5mol/L的舒必利溶液8次,发光强度的相对标准偏差(RSDs)为1.5%。该电极用于样品测定,回收率为97.6%～102.1%。结果表明,纳米金表现出较好的电分析活性,对联吡啶钌具有较好的电催化作用,并可应用于舒必利药物的测定。     

毛细管电泳-间接电化学发光法对茶叶中百草枯农药残留的检测

基于农药百草枯对钌联吡啶-三丙胺(TPA)体系的电化学发光具有显著的抑制作用,建立了毛细管电泳-间接电化学发光检测茶叶中残留农药百草枯的新方法.讨论了初始电位、钌联吡啶和TPA浓度、进样电压、进样时间、运行缓冲溶液的浓度与pH值等条件对百草枯检测灵敏度的影响.确定最佳实验条件为1.20 V初始电压、0.7 mmol/L钌联吡啶、0.6 mmol/L TPA、9 kV进样电压、9 s进样时间、35 mmol/L磷酸盐(pH 8.5)为运行缓冲溶液.在优化实验条件下,百草枯浓度在5×10~(-7) 5×10~(-5)mol/L范围内呈良好线性(相关系数为0.994 5),检出限为9.4×10~(-8) mol/L.对5×10~(-5) mol/L百草枯标准溶液连续测定5次,相对峰高与迁移时间的相对标准偏差分别为3.7%和2.1%.该方法对2.0×10~(-6)、1.0×10~(-5) mol/L百草枯标样的萃取回收率分别为74%和83%,相对标准偏差分别为15%、4.2%(n=5).     

基于壳聚糖/Ru（bpy）2+3/SiO2纳米粒子电化学发光传感器用于尿酸的检测

利用反相微乳液法制备了壳聚糖-Ru(bpy)2+3-SiO2复合纳米粒子,采用Nafion/MCNT复合膜技术实现了对复合纳米粒子有效而稳定的固定,从而制备了电化学发光传感器,实现了对尿酸的检测。在0.1 mol/L PBS缓冲溶液(pH 7.4)中,当尿酸与修饰电极作用15 min时,电化学发光强度与尿酸浓度(1.0×10-10~1.0×10-5 mol/L)的负对数呈良好的线性关系,线性方程为IECL=-709.52-202.74lgC,相关系数R=0.9936,检出限为6.0×10-12 mol/L。传感器表现出良好的重现性与稳定性,对1.0×10-8 mol/L尿酸平行测定11次,发光强度的相对标准偏差为2.9%,测定尿酸实际样品的加标回收率在98.5%~103.5%之间。     

基于Ru(bpy)_3~(2+)/AuNPs/Nafion电化学发光传感器检测己烯雌酚

利用柠檬酸钠还原氯金酸制得金纳米粒子(AuNPs),基于AuNPs/Nafion与Ru(bpy)_3~(2+)之间的静电引力,制备了Ru(bpy)_3~(2+)/AuNPs/Nafion电化学发光传感器。采用循环伏安法和电化学发光法对该传感器进行了表征,结果表明该传感器具有良好的稳定性和重现性,可实现对己烯雌酚的检测。在pH=7.0的0.1mol/L磷酸盐缓冲溶液(PBS,含0.05mol/L三正丙胺)中,当己烯雌酚与修饰电极作用15min时,电化学发光强度减少值与己烯雌酚浓度的负对数在1.0×10-10~5.0×10-7 mol/L范围内呈良好的线性关系,检出限为6.0×10-11 mol/L。对1.0×10-8 mol/L己烯雌酚平行测定11次,相对标准偏差为2.7%。测定己烯雌酚实际样品的加标回收率在98.0%~104.5%之间。     

CdSe量子点修饰电极电化学发光法测定叶酸

制备了水溶性的CdSe量子点,用紫外光谱和荧光光谱对其进行了表征.并将其修饰到金电极的表面,得到了CdSe量子点修饰电极(CdSe/GE),研究了其电化学发光性质.结果表明:在强碱介质中,CdSe/GE对鲁米诺电化学发光具有增敏作用,在此发光体系中加入叶酸后,会产生进一步增强的电化学发光信号,由此建立了电化学发光检测叶酸的新方法.考察了缓冲溶液pH值、鲁米诺的浓度和扫速等条件对电化学发光强度的影响.在优化的实验条件下,叶酸在1×10~(-13)~1.1×10~(-4) mol/L浓度范围内与相对发光强度(ΔI)呈现良好的线性关系,检测限为6.0×10~(-14) mol/L(S/N=3),并用于市售叶酸片剂中叶酸的测定,得到令人满意的实验结果.     

毛细管电泳安培法测定田基黄中的芦丁与槲皮素

建立了毛细管电泳电化学分离检测田基黄中生物活性成分芦丁和槲皮素的方法。考察了检测电极电位、缓冲液浓度、pH、运行电压和进样时间对分离的影响。以40 cm长,50μm内径的石英毛细管作为分离通道,运行缓冲液为25 mmol/L硼砂(pH 9.2)溶液,分离电压12 kV,0.3 mm直径的铂圆盘电极为检测电极,检测电位1.00 V(vs.Ag/AgCl),芦丁和槲皮素在10 min内得到良好分离。在上述实验条件下,芦丁和槲皮素分别在8.2×10-6~5.2×10-4mol/L与6.8×10-6~7.2×10-4mol/L范围内与峰面积呈良好线性关系,检出限分别为9.0×10-7mol/L(S/N=3)和4.7×10-7mol/L(S/N=3)。方法已应用于田基黄药材提取物成分分析。     

毛细管电泳-电致化学发光法测定兔血浆中的羟考酮

基于稀土Eu(Ⅲ)掺杂的类普鲁士蓝膜修饰的铂电极为工作电极,建立了测定羟考酮的毛细管电泳-电致化学发光分析方法。考察了检测电位、运行缓冲溶液的酸度及浓度、分离电压、进样条件等对电泳分离效果及检测灵敏度的影响。在最佳的实验条件下,羟考酮可在4 min内得到分离,其ECL强度值与羟考酮的质量浓度在7.0×10-2～7.0μg/mL和7.0～70.0μg/mL范围内呈良好的线性关系,检出限为4.2×10-2μg/mL(3σ),峰高和迁移时间的相对偏差分别为3.6%和0.48%(n=6)。方法用于兔血浆中羟考酮含量的检测,加标回收率在99.7%～101.0%之间。     

Analysis of amphetamines in urine with liquid-liquid extraction by capillary electrophoresis with simultaneous electrochemical and electrochemiluminescence detection

Amphetamines including methamphetamine, 3,4-methylenedioxyamphetamine and 3,4-methylenedioxymethamphetamine were separated and detected by CE using simultaneous electrochemical (EC) and electrochemiluminescence (ECL) detection (CE-EC/ECL). Factors that influenced the separation and detection performance, such as the detection potential, the pH value and concentration of the running buffer, the separation voltage and the pH of the detection buffer, were investigated. LODs of 3.3x10(-8) mol/L (0.16 fmol), 1.6x10(-7) mol/L (0.78 fmol) and 3.3x10(-8) mol/L (0.16 fmol) were obtained for methamphetamine, 3,4-methylenedioxyamphetamine and 3,4-methylenedioxymethamphetamine, respectively. For practical application, a liquid-liquid extraction with ethyl acetate procedure was developed for urine sample pretreatment and extraction efficiencies higher than 90% were obtained. The established simultaneous CE-EC/ECL was successfully applied for urine sample analysis.     

Determination of galanthamine in Bulbus Lycoridis Radiatae by coupling capillary electrophoresis with end‐column electrochemiluminescence detection

A novel method for the determination of galanthamine (GAL) in Bulbus Lycoridis Radiatae has been developed based on coupling CE with an end‐column tris(2,2′‐bipyridyl)ruthenium(II) electrochemiluminescence (ECL). Parameters affecting CE separation and ECL detection were investigated and optimized. Baseline separation of GAL from other components in the Bulbus Lycoridis Radiatae sample was achieved with an 18 mmol/L phosphate running buffer at pH 9.0. Under the optimized conditions: 12 kV CE‐separation voltage, ECL detection potential at 1.25 V with 5 mmol/L and 50 mmol/L phosphate buffer at pH 7.5 in the detection reservoir, the linear range of GAL concentration was from 0.8 ng/mL to 2 μg/mL, whereas the detection limit was 0.25 ng/mL (S/N=3). The proposed method was successfully demonstrated for the determination of GAL in Bulbus Lycoridis Radiatae.     

Optimization using central composite design for antihistamines separation by nonaqueous capillary electrophoresis with electrochemical and electrochemiluminescence detections

The first detailed examination of non-aqueous capillary electrophoresis with electrochemical and electrochemiluminescence detections (NACE-EC/ECL), separation parameters and their interactions via central composite design was presented. This concept was demonstrated by examining the optimization separation conditions of seven antihistamines (chlorpheniramine, cyproheptadine, diphenhydramine, doxylamine, methapyrilene, terfenadine, and triprolidine) by NACE-EC/ECL. To evaluate the NACE separation quality, the chromatography resolution statistic function (CRS(-1) function) with regard to the resolution and migration time was established as the response variable. The influences of three experimental variables (buffer apparent pH value (pH*), buffer (TBAP) concentration, and separation voltage) on the response were investigated. A set of optimal conditions was obtained from central composite design: 9.2 mM TBAP in ACN (pH* 4.0) and voltage (12.7 kV), and under these optimum conditions, the seven antihistamines could be well separated in less than 10 min. The obtained electropherograms indicated that the dual EC/ECL detection system was indispensable since the six antihistamines (except for triprolidine) displayed both EC and ECL response, whereas triprolidine only displayed the EC response. This work is instructive for investigators in simplifying the NACE-EC/ECL development procedures for multi-component analysis.     

Direct tris(2,2'-bipyridyl)ruthenium (II) electrochemiluminescence detection of polyamines separated by capillary electrophoresis

Capillary electrophoresis (CE) with tris(2,2'-bipyridyl) ruthenium (II) (Ru(bpy)3(2+)) electrochemiluminescence (ECL) detection technique was developed for the analysis of four polyamines (putrescine (Put), cadaverine (Cad), spermidine (Spd), and spermine (Spm)) analysis. The four polyamines contain different amine groups, which have different ECL activity. There are several parameters which influence the resolution and ECL peak intensities, including the buffer pH and concentrations, separation voltage, sample injection, electrode materials, and Ru(bpy)3(2+) concentrations. Polyamines are separated by capillary zone electrophoresis in an uncoated fused-silica capillary (50 cmx25 micro m (ID) filled with acidic phosphate buffer (200 mmol/L phosphate, pH 2.0) - 1mol/L phosphoric acid (9:1 v/v) and a separation voltage of 5 kV (25 micro A), with end-column Ru(bpy)3(2+) ECL detection. A 5 mmol/L Ru(bpy)3(2+) solution plus 200 mmol/L phosphate buffer (pH 11.0) is added into the reagent reservoir. The calibration curve is linear over a concentration range of two or three orders of magnitude for the polyamines. The analysis time is less than 25 min. Detection limits for Put and Cad are 1.9x10(-7) mol/L and 7.6x10(-9) mol/L for Spd and Spm, respectively. Intraday and interday relative standard deviations of ECL peak intensities are less than 8%. The main advantages of this CE-ECL detection technique for polyamines analysis presented herein are the omission of chemical derivatization of the analytes and the high selectivity.     

毛细管电泳电致化学发光检测血浆中布比卡因

布比卡因是一种外科局部麻醉剂,使用过量会导致中枢神经系统和心脏血管系统中毒^[1],可引起心脏停博.高效液相色谱和毛细管电泳(CE)^[2]是该药常用的检测方法.     

毛细管电泳-电致化学发光法测定土壤中的多抗霉素B

以稀土铕离子(Ⅲ)掺杂的类普鲁士蓝膜(Eu-PB)修饰铂电极为工作电极,采用毛细管电泳-电致化学发光法(CE-ECL)对土壤中的多抗霉素B进行检测.分别对毛细管电泳分离条件和电致化学发光检测条件进行优化,并探讨了体系产生电致化学发光的机理.在优化实验条件下,多抗霉素B可在4 min内得到分离,其ECL强度值与多抗霉素B...     

高效毛细管电泳电导法拆分苯丙氨酸对映体

以未涂层融硅石英毛细管(50 cm×75μm)为分离柱,2 mmol/L NaAc 2 mmol/L HAc 0.5 mmol/LCu2 (pH 4.0)作为电泳运行液,分离电压15 kV,建立了苯丙氨酸对映体的高效毛细管电泳-电导分离检测的方法。对缓冲溶液的种类、浓度、分离电压、有机改性剂等因素对分离的影响进行了讨论,并对拆分机理进行了初步探讨。     

毛细管电泳电致化学发光法同时测定氯丙嗪、异丙嗪及其主要代谢物

建立了同时检测氯丙嗪、异丙嗪及其主要代谢物的毛细管电泳电致化学发光新方法。最佳实验条件为: 检测电位1.20 V,钌联吡啶浓度5 mmol/L,检测池磷酸缓冲溶液40 mmol/L (pH 6.5),分离磷酸缓冲溶液18 mmol/L (pH 4.8),进样电压11 kV,进样时间8 s,分离电压13.5 kV。方法的检出限(3σ)分别为氯丙嗪8.3×10~7 g/L、异丙嗪7.2×10~6 g/L、氯丙嗪亚砜1.9×10~5g/L和异丙嗪亚砜3.7×10~6g/L,各组分的电化学发光强度和迁移时间的相对标准偏差(RSD)分别不超过3%和1%。本方法具有简便、快速、灵敏、进样量少和不受共存物干扰等特点,可在不必预分离的情况下直接同时连续测定家犬尿样中的氯丙嗪、异丙嗪、氯丙嗪亚砜和异丙嗪亚砜。