血红蛋白在溶胶-凝胶纳米银修饰电极上的直接电化学

运用溶胶-凝胶技术将血红蛋白(Hb)固定于纳米银(AgNPs)修饰的玻碳电极(GCE)表面,制得溶胶-凝胶血红蛋白纳米银修饰电极(Sol-Gel/Hb/AgNPs/GCE)。优化了修饰电极的制备条件,研究了该修饰电极在B-R缓冲溶液(pH=4.10)中的电化学行为,探讨了Hb在AgNPs修饰电极表面的直接电子转移机理。结果表明:AgNPs不仅保持了Hb的生物活性,而且通过它的催化效应,实现了Hb与电极之间的直接电子转移。进一步的实验结果显示,固定在纳米银修饰电极表面的Hb能保持其对H2O2的生物电催化活性。     

血红蛋白和SiO2凝胶层层组装膜在碳纳米管/金纳米粒子修饰电极界面上的直接电化学及电催化研究

以SiO2凝胶膜和蛋白质交互组装法固定血红蛋白(Hb), 对其进行了电化学和电催化研究. 首先制备碳纳米管/金纳米粒子复合材料修饰的MWNTs-Au/GC电极, 为防止蛋白质在电极表面流失, 将Hb和自制的SiO2凝胶膜交替滴涂到电极表面, 得到SiO2/Hb层层组装膜修饰电极, 即{SiO2/Hb}n/MWNTs-Au/GC电极, n=2为优化层数. Hb在{SiO2/Hb}2/MWNTs-Au/GC电极上仍能保持其特有的生物活性, 并能与电极进行稳定快速的电子直接转移, 同时表现出过氧化物酶特性, 对H2O2具有良好的生物电催化还原能力.     

对苯二胺在血红蛋白/聚L-谷氨酸/玻碳修饰电极上的可逆氧化

采用电聚合法在玻碳电极(GCE)表面得到导电性能良好的聚L-谷氨酸(PGA)薄膜,通过共价键合法将血红蛋白(Hb)固定于电极表面得到稳定且具有催化活性的Hb/PGA/GCE修饰电极,将其用于对苯二胺(PPD)的可逆氧化。 修饰电极交流阻抗及血红蛋白直接电化学实验表明,血红蛋白成功地固定于电极表面,保持良好的电催化活性,能有效催化H₂O₂的还原。 PPD在电极上表现为受吸附控制的准可逆氧化还原反应,I_p,a/I_p,c约为1.02,电极没有明显的钝化现象。 氧化还原峰电流与PPD的浓度均呈良好的线性关系,I_p,a(μA)=3.124+0.705c_PPD(mmol/L)(r=0.9973)。 H₂O₂的存在使PPD氧化还原峰型更对称,可逆性更好,表明体系中PPD氧化与过氧化酶催化途径一致。     

金复合介孔SBA-15吸附血红蛋白在H2O2电催化反应中的应用

以P123嵌段共聚物表面活性剂为模板剂制备介孔氧化硅SBA-15,并用沉积-沉淀(DP)法在SBA-15介孔表面负载纳米Au颗粒制备得到金复合介孔SBA-15材料(Au-SBA-15).再以Au-SBA-15材料制备玻碳修饰电极,将血红蛋白固定于修饰电极上用循环伏安法考察其对不同浓度H₂O₂溶液的电催化反应.在固定了血红蛋白的Hb/Au-SBA-15/GC修饰电极上,H₂O₂在+0.95 V处出现了氧化峰,且随着H₂O₂浓度的增大峰电流不断增加,说明金复合介孔氧化硅材料具有良好的生物兼容性,有利于血红蛋白的固定,其修饰电极对H₂O₂溶液具有一定的电催化作用.     

金复合介孔SBA-15吸附血红蛋白在H2O2电催化反应中的应用

以P123嵌段共聚物表面活性剂为模板剂制备介孔氧化硅SBA-15,并用沉积-沉淀(DP)法在SBA-15介孔表面负载纳米Au颗粒制备得到金复合介孔SBA-15材料(Au-SBA-15).再以Au-SBA-15材料制备玻碳修饰电极,将血红蛋白固定于修饰电极上用循环伏安法考察其对不同浓度H2O2溶液的电催化反应.在固定了血红蛋白的Hb/Au-SBA-15/GC修饰电极上,H2O2在+0.95 V处出现了氧化峰,且随着H2O2浓度的增大峰电流不断增加,说明金复合介孔氧化硅材料具有良好的生物兼容性,有利于血红蛋白的固定,其修饰电极对H2O2溶液具有一定的电催化作用.     

一种比率型Cu~(2+)电化学传感器及其分析应用

本研究以硫堇聚合物作为内参比探针分子,通过电化学聚合法将硫堇聚合于单壁碳纳米管修饰玻碳电极(SWNTs/GCE)上,并以该修饰电极为工作电极,建立了一种比率型检测Cu~(2+)的电化学传感方法。结果表明,在1~25μmol/L浓度范围内,Cu~(2+)的阳极溶出峰电流ICu~(2+)与聚硫堇氧化峰电流ITh的比值与Cu~(2+)浓度呈较好的线性关系,检测限为96nmol/L,方法用于加标自来水样中Cu~(2+)的检测,回收率较好。     

基于血红蛋白/金纳米粒子/聚二烯丙基二甲基氯化铵-多壁碳纳米管生物传感器测定过氧化氢

将分散于聚二烯丙基二甲基氯化铵(PDDA)中的多壁碳纳米管(MWCNT′s)滴涂在玻碳电极(GCE)表面制成PDDA-MWCNT′s/GCE修饰电极(简称电极Ⅰ);在氯金酸溶液中用恒电位沉积法使金纳米颗粒(AuNP′s)积镀于电极Ⅰ表面,制得AuNP′s/PDDA-MWNCT′s/GCE修饰电极(简称电极Ⅱ);将血红蛋白(Hb)滴于电极Ⅱ表面,用磷酸盐缓冲溶液冲洗后制成可供测定过氧化氢用的生物传感器Hb/AuNP′s/PDDA-MWCNT′s/GCE(简称电极Ⅲ)。与裸GCE、电极Ⅰ和Ⅱ相比较,在pH 6.8的磷酸盐缓冲溶液中,过氧化氢在电极Ⅲ上的还原峰电流明显提高,其值与过氧化氢浓度在1.0～1 800μmol.L-1范围内呈线性关系,其检出限(3S/N)为0.8μmol.L-1。应用此生物传感器测定消毒液中过氧化氢的含量,测定值与高锰酸钾滴定法的测定值相符。     

DNA电化学生物传感器在转基因植物特定序列基因检测中的应用

在玻碳电极(GCE)上采用循环伏安法电聚合硫堇(PTh)得到PTh/GCE修饰电极,并利用聚硫堇层共价结合和静电作用吸附金纳米粒子(AuNP′s)制得AuNP′s/PTh/GCE修饰电极。然后通过将ss-DNA/AuNP′s/PTh修饰电极置于cDNA杂交液中,于42℃杂交制得ds-DNA/AuNP′s/PTh修饰玻碳电极,实现了脱氧核糖核酸(DNA)探针在AuNP′s/PTh修饰的玻碳电极上的固定,制得DNA电化学生物传感器。在[Fe(CN)6]3-/4-溶液中采用微分脉冲伏安法(DPV)及交流阻抗谱技术(EIS)对DNA的固定和杂交进行了表征。试验结果表明:在1.0×10-10～1.0×10-6mol.L-1的浓度范围内,该传感器可对转基因植物外源基因草丁膦乙酰转移酶基因(PAT基因)片段进行检测,检出限(3s)为3.2×10-11mol.L-1。     

基于血红蛋白-纳米磷酸钬复合材料的过氧化氢生物传感器

以Ho2O3为反应物,采用水热法制备了纳米磷酸钬(n-HoPO4),并利用场发射扫描电子显微镜(SEM)、能谱分析(EDS)对其进行形貌表征和元素组成分析.将n-HoPO4和血红蛋白(Hb)复合材料修饰于裸玻碳电极(GCE)表面构建生物传感器,实现了对H2O2的电化学检测.采用循环伏安(CV)和电化学交流阻抗(EIS)技术对修饰电极进行表征,结果表明,Hb/n-HoPO4/GCE对H2O2的还原具有良好的电化学催化效果;n-HoPO4具有良好的导电性和生物相容性,促进了Hb与工作电极间的直接电子转移.研究了不同pH值和电化学扫速对修饰电极响应电流的影响.在优化实验条件下,此生物传感器对H2O2在50 ～ 1000 μmol/L范围内表现出良好的线性关系,相关线性系数R=0.999,检出限为17 μmol/L(S/N=3).此生物传感器具有检测范围宽、稳定性和重现性好、抗干扰能力强等优点,可用于实际样品的检测.     

电聚合构建HRP传感器检测有机过氧化物

利用电化学还原氧化石墨烯(GO)的方法将还原石墨烯(erGO)沉积在电极表面上,然后电沉积氧化锌纳米棒(ZnO)构成erGO/ZnO复合纳米材料修饰玻碳电极(GCE),最后通过电聚合中性红(NR)电子介体包埋法将辣根过氧化物酶(HRP)固定在GCE/erGO/ZnO表面制得GCE/erGO/ZnO/HRP-PNR(聚中性红)。用SEM和能谱对复合纳米材料进行了表征,通过电化学阻抗法和循环伏安法对修饰电极进行了探究,通过循环伏安法和计时电流法研究了GCE/erGO/ZnO/HRP-PNR对有机过氧化物的催化性能,结果该修饰电极对过氧化氢叔丁基(BHP)和过氧化氢异丙苯(CHP)都具有良好的检测性能。     

血红蛋白在壳聚糖修饰碳纳米管上的电化学特性及对过氧化氢的电催化分析

用壳聚糖对多壁碳纳米管进行修饰,构建了一种用于固定血红蛋白的新型复合材料,并研究了血红蛋白在该碳纳米管上的电化学性质及其对过氧化氢的电催化活性.扫描电镜结果表明,壳聚糖修饰的多壁碳纳米管呈单一的纳米管状,并能均匀分散在玻碳电极表面.紫外光谱分析表明血红蛋白在该复合膜内能很好地保持其原有的二级结构.将该材料固定在玻碳电极上后,血红蛋白能成功地实现其直接电化学.根据峰电位差随着扫描的变化,计算得到血红蛋白在壳聚糖修饰的碳纳米管膜上的电荷转移系数为0.57,表观电子转移速率常数为7.02 s-1.同时,该电极对过氧化氢显示出良好的催化性能,电流响应信号与H2O2浓度在1.0×10-6 ～1.5×10-3 mol/L间呈线性关系,检出限为5.0×10-7 mol/L.修饰电极显示了良好的稳定性.     

血红蛋白在纳米孔径氧化铝膜修饰电极上的直接电化学

运用电化学包埋法成功将血红蛋白(Hb)固定于纳米孔阳极氧化铝膜(AAO)修饰的玻碳电极(GC)表面, 制得Hb/PPy/AAO/GC修饰电极, 并对Hb/PPy/AAO/GC修饰电极的制备条件进行了优化. 研究了Hb/PPy/AAO/GC修饰电极在磷酸缓冲液(pH＝6.8)中的电化学行为, 探讨了血红蛋白在AAO修饰电极表面的直接电子转移机理. 结果表明阳极氧化铝膜不仅保持了血红蛋白的生物活性, 而且通过它的纳米尺寸效应, 实现了Hb与电极之间的直接电子转移. 其研究内容对生命科学和临床医学有着重要意义.     

Amperometric biosensor for hydrogen peroxide based on direct electrocatalysis by hemoglobin immobilized on gold nanoparticles/1,6-diaminohexane modified glassy carbon electrode.

A facile strategy of an amperometric biosensor for hydrogen peroxide based on the direct electrocatalysis of hemoglobin (Hb) immobilized on gold nanoparticles (GNPs)/1,6-diaminohexane (DAH) modified glassy carbon electrode (GCE) has been described. A uniform monolayer film of DAH was initially covalently bound on a GCE surface by virtue of the electrooxidation of one amino group of DAH, and another amino group was modified with GNPs and Hb, successively. The fabrication process was characterized by cyclic voltammetry (CV), electrochemical impedance spectroscopy (EIS) and scanning electron microscopy (SEM). The proposed biosensor exhibited an effective and fast catalytic response to the reduction of H2O2 with good reproducibility and stability. A linear relationship existed between the catalytic current and the H2O2 concentration in the range of 1.5x10(-6) to 2.1x10(-3) M with a correlation coefficient of 0.998 (n=24). The detection limit (S/N=3) was 8.8x10(-7) M.     

Application of Titanium Dioxide Nanowires for the Direct Electrochemistry of Hemoglobin and Electrocatalysis

Titanium dioxide (TiO₂) nanowires were synthesized and used for the realization of direct electrochemistry of hemoglobin (Hb) with carbon ionic liquid electrode (CILE) as the substrate electrode. TiO₂‐Hb composite was casted on the surface of CILE with a chitosan film and spectroscopic results confirmed that Hb retained its native structure in the composite. Direct electron transfer of Hb on the modified electrode was realized with a pair of quasi‐reversible redox waves appeared, indicating that the presence of TiO₂ nanowires could accelerate the electron transfer rate between the electroactive center of Hb and the substrate electrode. Electrochemical behaviors of Hb on the modified electrode were carefully investigated with the values of the electron transfer coefficient (α), the electron transfer number and the heterogeneous electron transfer rate constant (k_s) as 0.58, 0.98 and 1.62 s^‐1. The Hb modified electrode showed excellent electrocatalytic activity to the reduction of trichloroacetic acid and NaNO₂ with wider linear range and lower detection limit, indicating the successful fabrication of a new third‐generation biosensor.     

基于中空氧化镍纳米微球和离子液体复合膜固定血红蛋白的NaNO2生物传感器

采用微波水热法合成了一种中空氧化镍纳米微球(NiO), 然后将其与1-丁基-3-甲基-咪唑四氟硼酸盐(BMIMBF4)的复合膜用于血红蛋白(Hb)在碳糊电极上的固定, 制备了NaNO2生物传感器. 通过扫描电子显微镜、 傅里叶变换红外光谱及紫外-可见光谱等分析表明, Hb已固定于NiO和BMIMBF4的复合膜中并能保持其生物活性; 进一步通过电化学阻抗法研究了修饰电极中混合物各组分的作用. 结果表明, 在NiO和BMIMBF4的复合膜中, Hb能实现有效的直接电子转移, 且修饰后的电极对NaNO2有良好响应, 响应时间小于5 s, 检出限为4.57 μmol/L(S/N=3), 灵敏度为46.2 μA·L·mmol-1, 线性范围为10~170 μmol/L, 表观米氏常数KM为2.4 mmol/L, 该方法的重现性和电极的稳定性良好.     

Hemoglobin/colloidal silver nanoparticles immobilized in titania sol-gel film on glassy carbon electrode: direct electrochemistry and electrocatalysis

By vapor deposition method, both hemoglobin (Hb) and colloidal silver nanoparticles (CSNs) were entrapped in a titania sol-gel matrix on the surface of a glassy carbon electrode (GCE). CSNs could greatly enhance the electron transfer reactivity of Hb and its catalytic ability toward nitrite. Direct fast electron transfer between Hb and the GCE was achieved, and a pair of well-defined, quasi-reversible redox peaks was observed. The anodic and cathodic peak potentials are located at -0.298 V and -0.364 V (vs. Ag/AgCl), respectively. The dependence of the formal potential on solution pH indicated that the direct electron transfer reaction of Hb was a one-electron transfer coupled with a one-proton transfer reaction process. Meanwhile, the catalytic ability of Hb toward the reduction of NO2- was also studied. Accordingly, a NO2- biosensor was prepared, with a linear range from 0.2 mM to 6.0 mM and a detection limit of 34.0 microM. The apparent Michaelis-Menten constant was calculated to be 7.48 mM. Moreover, the biosensor had good long-term stability.     

Electrochemical Biosensor Based on Carbon Ionic Liquid Electrode Modified with Nafion/Hemoglobin/DNA Composite Film

A new electrochemical biosensor was constructed by immobilization of hemoglobin (Hb) on a DNA modified carbon ionic liquid electrode (CILE), which was prepared by using 1‐ethyl‐3‐methylimidazolium tetrafluoroborate (EMIMBF₄) as the modifier. UV‐vis absorption spectroscopic result indicated that Hb remained its native conformation in the composite film. The fabricated Nafion/Hb/DNA/CILE was characterized by scanning electron microscopy (SEM), electrochemical impedance spectroscopy (EIS) and cyclic voltammetry (CV). A pair of well‐defined redox peaks was obtained on the modified electrode, indicated that the Nafion and DNA composite film provided an excellent biocompatible microenvironment for keeping the native structure of Hb and promoting the direct electron transfer rate of Hb with the basal electrode. The electrochemical parameters of Hb in the composite film were further calculated with the results of the charge transfer coefficient (α) and the apparent heterogeneous electron transfer rate constant (k_s) as 0.41 and 0.31 s^?1. The proposed electrochemical biosensor showed good electrocatalytic response to the reduction of trichloroacetic acid (TCA), H₂O₂, NO and the apparent Michaelis–Menten constant (K_M^app) for the electrocatalytic reaction was calculated, respectively.     

A novel amperometric hydrogen peroxide biosensor based on electrospun Hb-collagen composite

In this paper, the hemoglobin (Hb)-collagen microbelt modified electrode with three-dimensional configuration was fabricated via the electrospinning method. Direct electron transfer of the Hb immobilized into the electrospun collagen microbelts was greatly facilitated. The apparent heterogeneous electron transfer rate constant (k(s)) was calculated to be 270.6s?1. The electrospun Hb-collagen microbelt modified electrode showed an excellent bioelectrocatalytic activity toward the reduction of H?O?. The amperometric response of the biosensor varied linearly with the H?O? concentration ranging from 5 × 10??molL?1 to 30×10??molL?1, with a detection limit of 0.37 × 10??molL?1 (signal-to-noise ratio of 3). The apparent Michaelis-Menten constant (K(m)(app)) was 77.7 μmolL?1. The established biosensor exhibited fast amperometric response, high sensitivity, good reproducibility and stability.     

基于聚硫堇/过氧化氢光电化学敏感界面的胆碱传感器

将胆碱氧化酶固定在具有光电活性的聚硫堇光透电极的表面,利用壳聚糖和戊二醛键合胆碱氧化酶制备了光致电化学胆碱传感器.此传感器基于同时具有光敏和电子受体功能的聚硫堇光电界面,能与胆碱氧化酶催化胆碱反应产生的电子供体(H2O2)发生光致电化学反应的原理,实现了对胆碱的检测.探讨了传感器的光致电化学响应机理、偏压、光强及电解质...     

铁氰化铈薄膜固载血红蛋白修饰的过氧化氢生物传感器的制备及性能

采用电化学沉积法将铁氰化铈(CeHCF)薄膜修饰于玻碳电极(GCE)表面,得到铁氰化铈薄膜修饰玻碳电极;将血红蛋白(Hb)固载于该修饰电极表面,成功制得了Hb/CeHCF/GCE过氧化氢生物传感器.考察了铁氰化铈薄膜修饰玻碳电极的氧化还原机理和制备条件,并对血红蛋白在电极上的电子传递过程进行了较为深入的研究.结果表明,铁氰化铈薄膜为血红蛋白提供了温和的固载环境,可实现血红蛋白与电极表面的直接电子转移,提高了血红蛋白的电化学活性;所制得的传感器对过氧化氢具有较高的催化响应和较强的稳定性.相关研究结果在生物医学和临床医学领域具有一定的借鉴意义.