聚钙羧酸修饰玻碳电极差分脉冲伏安法同时测定多巴胺和尿酸

采用电化学方法将钙羧酸(CCA)聚合修饰在玻碳电极(GCE)表面制备了聚钙羧酸指示剂修饰玻碳电极(PCCA/GCE),并用循环伏安法和交流阻抗法研究了电极的电化学性能。结果表明:在pH 6.0的磷酸盐缓冲溶液中,多巴胺(DA)和尿酸(UA)在聚钙羧酸修饰电极上的氧化峰得以分开,峰电位差为0.14V,据此提出了聚钙羧酸修饰电极差分脉冲伏安法同时测定多巴胺和尿酸的方法。DA和UA的浓度分别在5.0～43.8μmol.L-1和5.0～50.0μmol.L-1范围内与其氧化峰电流呈线性关系,检出限(3S/N)分别为0.2μmol.L-1和0.5μmol.L-1。方法可用于多巴胺注射液样品中DA和UA的测定,测定值的相对标准偏差(n=5)依次为2.43%和2.35%。     

镍纳米粒子-离子液体修饰碳糊电极的制备及其对多巴胺的测定

制备了镍纳米粒子-离子液体修饰电极,在0.1 mol/L磷酸缓冲溶液(pH 6.0)中研究了多巴胺(DA)在修饰电极上的电化学行为.与裸电极相比,DA在该修饰电极上的氧化还原电位明显降低,氧化还原反应的峰电流明显增大,DA的峰电流与其浓度在2.0×10~(-8) ～1.0×10~(-4) mol/L范围内呈良好的线性关系,检出限为6.5×10~(-9) mol/L.该修饰电极对抗坏血酸具有明显的抗干扰能力.     

TiO2-石墨烯-Nafion复合膜修饰玻碳电极同时测定多巴胺和尿酸

利用在玻碳电极上修饰了TiO2-石墨烯-Nafion复合膜制得的修饰电极进行多巴胺(DA)和尿酸(UA)的同时测定。用循环伏安法(CV)和差分脉冲伏安法(DPV)研究了该修饰电极的电化学行为。在pH为7.0的磷酸盐缓冲液(PBS)中,修饰电极对于DA和UA的电化学氧化具有良好的电催化性能。DA和UA的氧化峰电流分别在2～120和60～300μmol/L浓度范围内呈良好的线性关系,检出限分别为0.066和0.102μmol/L。实验结果表明,TiO2-石墨烯-Nafion复合膜修饰电极显著提高了检测的灵敏度,并表现出良好的选择性和重现性。     

电还原柠嗪酸修饰电极对多巴胺和尿酸的电化学性质研究

采用循环伏安法制备了电还原柠嗪酸膜修饰碳糊电极(ECA/CPE),研究了多巴胺(DA)在该修饰电极上的电化学行为。在pH 7.0的磷酸盐缓冲溶液中,ECA/CPE对DA具有明显的电催化作用,且DA呈现出一对准可逆的氧化还原峰,其氧化峰电流与DA浓度在3.7×10-7~8.2×10-5mol/L和1.04×10-4~9.34×10-4mol/L范围内呈良好的线性关系,检出限为1×10-7mol/L(S/N=3)。使用微分脉冲伏安法,DA和尿酸(UA)在ECA/CPE上的氧化峰能完全分离,且峰电流与浓度呈良好的线性关系。该电极可用于盐酸多巴胺针剂中DA的测定以及人体尿液中UA的检测。     

聚氨基黑10B/Nafion修饰电极上多巴胺的检测

用电化学聚合法制备了聚氨基黑10B/Nafion修饰电极,利用循环伏安法研究了多巴胺在此修饰电极上的电化学行为.在磷酸盐缓冲溶液(pH 6.0)中,多巴胺在修饰电极上呈现可逆的氧化还原峰.其峰电位都随pH值的增加而负移.多巴胺氧化还原峰电流与其浓度在0.2～30 μmol/L范围内呈良好的线性关系;检出限为1.0×10~7 mol/L.实验结果表明:本修饰电极具有良好的重现性、稳定性和较强的抗干扰能力.将此修饰电极用于多巴胺注射液和小牛血清中多巴胺的检测,结果令人满意.     

单分子层γ-氨基丁酸共价修饰玻碳电极同时测定多巴胺、尿酸和抗坏血酸

采用电氧化法制备了一种新型γ-氨基丁酸(ABA)修饰的玻碳电极.X射线光电子能谱(XPS)和循环伏安法研究表明,ABA以单分子层状态以C—N键牢固地共价键合在电极表面.该修饰电极对多巴胺(DA)、尿酸(UA)和抗坏血酸(AA)都具有良好的电化学催化特性.在pH=7.0磷酸缓冲溶液中,DA,UA和AA分别于0.45,0.25和0.07V(vs.Ag/AgCl)有一个良好的、独立的阳极方波伏安峰,表明此修饰电极可用于这3种物质的同时测定.与DA,UA和AA的方波伏安峰电流呈线性关系的浓度范围分别为4.0～400,2.0～500和1.0～600μmol/L,检测限(3δ)分别为1.6,1.2和0.8μmol/L.该修饰电极具有良好的灵敏度、选择性和稳定性,并具有抗污染能力.     

纳米NiO-还原石墨烯复合修饰玻碳电极的制备及电催化检测多巴胺

制备了纳米NiO-还原石墨烯复合修饰电极(NiO-rGO/GCE),并用于多巴胺(DA)的检测。用循环伏安法(CV)和差分脉冲伏安法(DPV)研究了DA在该修饰电极上的电化学行为。结果表明,在pH=7.0的磷酸盐缓冲溶液(PBS)中,该修饰电极对DA有良好的催化作用。DA浓度在5.0×10-7~3.2×10-5 mol/L范围内与氧化峰电流呈良好的线性关系,检出限为3.8×10-8 mol/L。用该修饰电极直接测定了血清中DA含量,回收率在97.8%~101.1%之间。     

尿酸在有序介孔碳-壳聚糖修饰电极上的电化学行为及其测定

用硬模板法合成了有序介孔碳(OMC),并以壳聚糖(Chitosan)作为分散剂制备了有序介孔碳-壳聚糖复合膜(OMC-Chitosan)修饰电极.应用该电极研究了尿酸(UA)的电化学行为以及实际样品的分析检测.在0.1 mol/L(pH 6.5)的磷酸盐(PBS)缓冲溶液中,UA在OMC-Chitosan修饰电极上于0.334 V处产生一灵敏的不可逆氧化峰,氧化峰电流(ipa)与UA的浓度在4.0×10-6～2.0×10-4 mol/L范围内呈良好的线性关系,相关系数为0.9997,检出限为2.0×10-6 mol/L.对0.2 mmol/L UA平行测定10次,相对标准偏差为3.8%,表明该电极重现性和稳定性良好.     

尿酸在石墨烯修饰玻碳电极上的电化学行为及测定

以抗坏血酸为还原剂,采用微波水热法化学还原氧化石墨烯合成了石墨烯纳米片,制备了石墨烯修饰的玻碳电极(RGO/GCE),并采用循环伏安法、计时电量法、交流阻抗法等电化学技术研究了尿酸在该修饰电极上的电化学行为及其影响因素。结果表明,在PBS缓冲溶液中,尿酸(UA)在石墨烯修饰电极上的电极反应是一个受扩散控制的不可逆氧化过程。电极反应的转移电子数n=2,有效面积A=0.182 cm2,扩散系数D=1.51×10-6 cm2.s-1。UA的氧化峰电流与其浓度在5.0×10-6～1.5×10-4 mol/L范围内呈良好线性,r=0.995 7。利用该RGO/GCE修饰电极可以快速准确地测定UA,检出限为2.7×10-7 mol/L,加标回收率为98%～100%。     

氮掺杂石墨烯与发夹DNA修饰的电极为工作电极-差分脉冲伏安法用于测定多巴胺

将玻碳电极(GCE)打磨至呈镜面,在其表面上滴加氮掺杂石墨烯悬浮液5.0μL,在50℃的红外灯下烘干,制得氮掺杂石墨烯修饰的GCE;然后取5.0μmol·L-1发夹DNA(H DNA)溶液10μL滴涂于氮掺杂石墨烯修饰电极表面,制得氮掺杂石墨烯和H DNA修饰的GCE。用此修饰电极作为工作电极,用差分脉冲伏安法(DPV)测定人体血清中多巴胺(DA)的含量。试验表明:氮掺杂石墨烯和H DNA修饰的电极对DA的电化学氧化具有更好的电催化作用。DA在此修饰电极上的氧化峰电流与其浓度在4.0×10-7～6.0×10-5 mol·L-1内呈线性关系,检出限(3s/k)为6.6×10-8 mol·L-1。测定时用pH 6.5磷酸盐缓冲溶液(PBS)作为支持电解质。分析血清样品时前处理如下:取血清样品2.0mL,加入甲醇4.0mL,离心沉淀。取上清液2.0mL,加入等体积的pH 6.5PBS,充分混匀后供测定。用pH 6.5的PBS配制DA标准溶液系列,利用DPV对DA标准溶液系列进行测定,记录其氧化峰电流值,制作工作曲线。应用此方法分析了人体血清样品并以此样品为基体进行加标回收试验,测得回收率在90.0%～110%之间,测定值的相对标准偏差(n=5)在1.7%～3.7%之间。     

Electropolymerization of Thin Film Conducting Polymer and Its Application for Simultaneous Determination of Ascorbic Acid,Dopamine and Uric Acid

In this paper electropolymerization of a thin film of para‐phenylenediamine (PPD) is studied at glassy carbon electrode (GCE) in sulfuric acid media by cyclic voltammetry. The results showed that this polymer was conducting and had a reproducible redox couple in the potential region from 0.0 to 0.4 V in phosphate buffer solution. This modified GCE (p‐PPD‐GCE) was applied for simultaneous determination of ascorbic acid (AA), dopamine (DA) and uric acid (UA) using differential pulse voltammetry (DPV). The p‐PPD‐GCE in 0.1 M phosphate buffer solution (pH 5.0) separated the DPV signals of AA, DA and UA with sufficient potential differences between AA–DA and DA–UA and also enhanced their oxidation peak currents. The oxidation currents were increased from 2.0 to 2000.0 µM for AA, 10.0 to 1250.0 µM for DA and 50.0 to 1600.0 µM for UA. The detection limits were evaluated as 0.4, 1.0 and 2.5 µM for AA, DA and UA, respectively (S/N=3).     

Selective Detection of Uric Acid in the Presence of Ascorbic Acid and Dopamine Using Polymerized Luminol Film Modified Glassy Carbon Electrode

Electrochemically polymerized luminol film on a glassy carbon electrode (GCE) surface has been used as a sensor for selective detection of uric acid (UA) in the presence of ascorbic acid (AA) and dopamine (DA). Cyclic voltammetry was used to evaluate the electrochemical properties of the poly(luminol) film modified electrode. Scanning electron microscopy (SEM) and atomic force microscopy (AFM) have been used for surface characterizations. The bare GCE failed to distinguish the oxidation peaks of AA, DA and UA in phosphate buffer solution (pH 7.0), while the poly(luminol) modified electrode could separate them efficiently. In differential pulse voltammetric (DPV) measurements, the modified GCE could separate AA and DA signals from UA, allowing the selective determination of UA. Using DPV, the linear range (3.0×10^?5 to 1.0×10^?3 M) and the detection limit (2.0×10^?6 M) were estimated for measurement of UA in physiological condition. The applicability of the prepared electrode was demonstrated by measuring UA in human urine samples.     

抗坏血酸和尿酸在甘氨酸-壳聚糖修饰玻碳电极上的电化学行为及测定

制备了甘氨酸-壳聚糖复合膜修饰玻碳电极(Gly-CTS/GCE),研究了抗坏血酸(AA)和尿酸(UA)在该修饰电极上的电化学行为。结果表明在pH=5.59的磷酸盐缓冲溶液中,AA、UA在Gly-CTS/GCE上均产生灵敏的不可逆氧化峰,其峰电流与浓度在一定范围内呈良好的线性关系。对AA和UA混合溶液平行测定7次,相对标准偏差分别为4.6%、2.9%,表明该电极重现性和稳定性良好。AA、UA在Gly-CTS/GCE电极上的氧化峰峰电位相差340mV,据此可实现对二者的同时检测,并可应用于实际样品测定。     

用聚(L-蛋氨酸)/纳米金修饰玻碳电极同时灵敏检测多巴胺和尿酸简

A novel electrochemical sensor was fabricated by electrodeposition of gold nanoparticles on a poly(L-methionine) (PMT)-modified glassy carbon electrode (GCE) to form a nano-Au/PMT composite-modified GCE (nano-Au/PMT/GCE). Scanning electron microscopy and electrochemical techniques were used to characterize the composite electrode. The modified electrode exhibited considerable electrocatalytic activity towards the oxidation of dopamine (DA) and uric acid (UA) in phosphate buffer solution (pH = 7.00). Differential pulse voltammetry revealed that the electrocatalytic oxidation currents of DA and UA were linearly related to concentration over the range of 5.0×10^-8 to 10^-6 mol/L for DA and 7.0×10^-8 to 10^-6 mol/L for UA. The detection limits were 3.7×10^-8 mol/L for DA and 4.5×10^-8 mol/L for UA at a signal-to-noise ratio of 3. According to our experimental results, nano-Au/PMT/GCE can be used as a sensitive and selective sensor for simultaneous determination of DA and UA.     

聚对氨基苯磺酸/石墨烯复合修饰电极对尿酸的选择性灵敏测定

采用电聚合方法在石墨烯纳米片(GN)的表面聚合一层聚对氨基苯磺酸(PABSA),制备了聚对氨基苯磺酸/石墨烯复合修饰玻碳电极(PABSA/GN/GCE)。研究了尿酸(UA)和抗坏血酸(AA)在该修饰电极上的电化学行为。与聚对氨基苯磺酸修饰电极(PABSA/GCE)及石墨烯单层膜修饰电极(GN/GCE)相比,复合修饰电极PABSA/GN/GCE显著提高了对UA和AA的检测灵敏度和分离度。在0.1 mol/L磷酸盐缓冲溶液(pH7.0)中,UA和AA的峰电位差达344 mV,表明PABSA/GN/GCE能实现对UA的选择性测定。UA的峰电流与其浓度呈良好的线性关系,线性范围为1.0×10-7～8.0×10-4mol/L,检出限为4.5×10-8mol/L。该复合修饰电极用于尿样中尿酸的测定,结果满意。     

RNA Modified Electrodes for Simultaneous Determination of Dopamine and Uric Acid in the Presence of High Amounts of Ascorbic Acid

A promising electrochemical biosensor was fabricated by electrochemical grafting of ribonucleic acid (RNA) at 1.8 V (vs. SCE) on glassy carbon electrode (GCE) (denoted as RNA/GCE), for simultaneous detection of dopamine (DA) and uric acid (UA) with coexistence of excess amount of ascorbic acid (AA). The electrode was characterized by X‐ray photoelectron spectroscopy (XPS), cyclic voltammetry (CV) and differential pulse voltammetry (DPV) techniques. The RNA modified layer on GCE exhibited superior catalytic ability and anionic exclusive ability in comparison with the DNA modified electrode. Three separated anodic DPV peaks were obtained at 0.312, 0.168 and ?0.016 V for UA, DA and AA, respectively, at the RNA/GCE in pH 7.0 PBS. In the presence of 2.0 mM AA, a linear range of 0.37 to 36 μM with a detection limit of 0.2 μM for DA, and in the range of 0.74 to 73 μM with a detection limit of 0.36 μM for UA were obtained. The co‐existence of 5000 fold AA did not interfere with the detection of DA or UA. The modified electrode shows excellent selectivity, good sensitivity and good stability.     

Detection of Uric Acid in the Presence of Dopamine and High Concentration of Ascorbic Acid Using PDDA Modified Graphite Electrode

The properties of graphite electrode (Gr) modified with poly(diallyl dimethyl ammonium chloride) (PDDA) for the detection of uric acid (UA) in the presence of dopamine (DA) and high concentration of ascorbic acid (AA) have been investigated by cyclic voltammetry, differential pulse voltammetry and chronoamperometry. The polymer modified graphite electrode was prepared by a very simple method just by immersing the graphite electrode in PDDA solution for 20 minutes. The PDDA/Gr modified electrode displayed excellent electrocatalytic activity towards the oxidation of UA, DA and AA compared to that at the bare graphite electrode. The electrochemical oxidation signals of UA, DA and AA are well resolved into three distinct peaks with peak potential separations of 220 mV, 168 mV and 387 mV between AA‐DA, DA‐UA and AA‐UA respectively in cyclic voltammetry studies and the corresponding peak potential separations are 230 mV, 130 mV and 354 mV respectively in differential pulse voltammetry. The lowest detection limits obtained for UA, DA and AA were 1×10^?7 M, 2×10^?7 M and 800×10^?9 M respectively. The PDDA/Gr electrode efficiently eliminated the interference of DA and a high concentration of AA in the determination of UA with good selectivity, sensitivity and reproducibility. The modified electrode was also successfully applied for simultaneous determination of UA, DA and AA in their ternary mixture.