酶法合成的葡萄糖氧化酶-纳米金复合物的直接电化学与生物传感

将NaAuCl₄、葡萄糖氧化酶（GOx）和葡萄糖混合,借一步酶促反应制得吸附GOx的金纳米颗粒（AuNPs）,再通过滴干修饰法研制了Nafion/GOx-AuNPs修饰的玻碳（GC）电极,并考察了该酶电极上GOx的直接电化学和生物传感性能. 这种酶法合成的GOx-AuNPs复合物有良好的酶直接电化学活性,也保持了GOx的生物活性,似可归因于酶法合成的纳米金更接近酶氧化还原活性中心的缘故. 该酶电极在-0.4 V（vs. SCE）电位下,其稳态电流下降与葡萄糖浓度（0.5 4 mmol·L^-1）成正比,检测下限0.2 mol·L^-1.     

在离子液体[BMIm][BF4]中电沉积光亮金镀层

在离子液体1-丁基-3-甲基咪唑四氟硼酸盐（[BMIm][BF₄]）中以HAuCl₄·3H₂O为主盐、通过添加5,5-二甲基乙内酰脲（DMH）和胞嘧啶可得到色泽光亮、厚度达1.5 μm的金镀层,沉积过程中阴极电流效率可达到100%。SEM和XRD测试结果表明,DMH和胞嘧啶具有细化晶粒、平整镀层的作用。电化学测试结果表明,DMH可分别与Au³⁺、Au⁺形成配合物Au（DMH）₄^-、Au（DMH）₂^-,抑制了还原过程的表面转化步骤,从而增加了阴极极化,起到光亮镀层、细化晶粒的作用;胞嘧啶可在金核表面吸附,从而可以进一步光亮镀层、细化晶粒,与DMH有协同作用。循环伏安测试研究了镀液的电化学行为,研究表明在此体系中Au³⁺的还原为两步还原过程,分别为Au³⁺→ Au⁺和Au⁺→ Au。此外DMH和胞嘧啶的添加不会带来副反应。     

镀金和碳纳米管修饰金电极上吸附态葡萄糖氧化酶比活性的EQCM研究

采用石英晶体微天平(EQCM)技术监测了裸金电极、镀金和碳纳米管修饰金电极上葡萄糖氧化酶(GOD)的吸附过程. 通过EQCM测量吸附固定的GOD质量, 并实时检测酶反应产物H2O2的氧化电量, 求算了各表面上吸附态GOD的比活性(ESAi). 结果表明, 各表面上均可吸附一定的GOD, 且吸附态GOD均有一定的酶活性; 修饰CNTs可增大酶吸附量和酶电极对葡萄糖的响应电流, 但ESAi随CNTs修饰量的增大而降低; Au电极上电镀金后, 酶吸附量和酶电极对葡萄糖的响应电流亦增大, 但ESAi与裸金电极上的基本一致.     

Aun(n=2-9)团簇与乙醇分子相互作用的第一性原理研究

利用密度泛函理论研究了Au_n(n=2-9)团簇吸附一个乙醇分子的结构和电子性质. 研究结果表明: Au_n(n=2-9)团簇的最稳定构型为二维平面结构, Au6团簇最稳定; 吸附过程是通过金团簇上一个特定的金原子与乙醇分子中氧原子相互作用完成, 形成了20种稳定构型; 金原子的配位数对吸附作用影响明显; 作为吸附主体的金团簇和被吸附的乙醇分子在吸附前后构型无明显变化, 它们之间为弱相互作用.     

O与O2在Au团簇上吸附的密度泛函理论研究

采用基于密度泛函理论(DFT)的Dmol³程序系统研究了O原子与O₂在 Au₁₉与Au₂₀团簇上的吸附反应行为. 结果表明: O在Au₁₉团簇顶端洞位上的吸附较Au₂₀强; 在侧桥位吸附强度相近. O与O₂在带负电Au团簇上吸附较强, 在正电团簇吸附较弱. 从O―O键长看, 当金团簇带负电时, O―O键长较长, 中性团簇次之, 正电团簇中O―O键长较短, 因而O₂活化程度依次减弱. 电荷布居分析表明, Au团簇带负电时, O与O₂得电子数较中性团簇多, 而团簇带正电时, 得电子数较少. 差分电荷密度(CDD)表明, O₂与Au团簇作用时, 金团簇失电子, O₂的π^*轨道得电子, 使O―O键活化. O₂在Au₁₉^-团簇上解离反应活化能为1.33 eV, 较中性团簇低0.53 eV; 而在Au₁₉⁺上活化能为2.27 eV, 较中性团簇高0.41 eV, 这与O₂在不同电性Au₁₉团簇O―O键活化规律相一致.     

Au Nanowires-MWCNTs修饰电极对葡萄糖的催化氧化

通过油胺(Oleylamine)还原法制备了金纳米线(Au nanowires),将其与酸化处理的多壁碳纳米管(MWCNTs)通过层层组装制备了Au nanowires-MWCNTs复合结构修饰的玻碳电极(Au nanowires-MWCNTs/GCE).电化学研究结果表明,与单纯Au nanowires或MWCNTs修饰电极相比,Au nanowires-MWCNTs/GCE对葡萄糖表现出更优良的电催化性能.以Au nanowires-MWCNTs/GCE为阳极,电沉积Pt膜电极(Pt/GCE)为阴极,构建了葡萄糖/O2燃料电池.测试结果表明,构建的燃料电池的开路电位(OCP)为0.57 V,在0.44 V下最大功率密度(Pmax)为0.28 m W/cm2.     

SnO2负载Au和M-Au(M=Pt,Pd)催化剂及其低温催化氧化CO性能

以SnO₂为载体, 采用沉积沉淀法(DP)、共沉淀法(CP)和浸渍法(IM)制备了金负载Au/SnO₂催化剂, 同时采用沉积沉淀法制备了M-Au/SnO₂(M=Pd, Pt)双金属负载催化剂. 通过X射线衍射(XRD)、BET比表面积测定、透射电镜(TEM)和X射线光电子能谱(XPS)等技术对样品进行表征, 并测定其对CO的催化活性. 结果表明: 与CP法和IM 法相比, DP法制备的Au/SnO₂-DP 催化剂, Au 颗粒(<5 nm)较小, 分布均匀; Au/SnO₂-DP 中的Au 是以金属态Au0存在, 而Au/SnO₂-CP 和Au/SnO₂-IM 中, 金以Au⁰和Au³⁺的混合价态存在, 在Au/SnO₂-DP和M-Au/SnO₂中的Au、Pt、Pd和SnO₂之间存在相互作用; Au/SnO₂-DP 催化性能明显优于Au/SnO₂-CP 和Au/SnO₂-IM. Au与Pt 和Pd的双金属复合催化剂催化活性明显提高. 不同方法制备Au/SnO₂催化活性的差别主要是由于Au颗粒大小和Au氧化态的不同而产生. 而M-Au/SnO₂活性提高, 可能是由于Au与Pt 和Pd之间的相互作用.     

在离子液体[BMIm][BF4]中电沉积光亮金镀层

在离子液体1-丁基-3-甲基咪唑四氟硼酸盐（[BMIm][BF₄]）中以HAuCl₄·3H₂O为主盐、通过添加5,5-二甲基乙内酰脲（DMH）和胞嘧啶可得到色泽光亮、厚度达1.5 μm的金镀层,沉积过程中阴极电流效率可达到100%。SEM和XRD测试结果表明,DMH和胞嘧啶具有细化晶粒、平整镀层的作用。电化学测试结果表明,DMH可分别与Au³⁺、Au⁺形成配合物[Au（DMH）₄]^-、[Au（DMH）₂]^-,抑制了还原过程的表面转化步骤,从而增加了阴极极化,起到光亮镀层、细化晶粒的作用;胞嘧啶可在金核表面吸附,从而可以进一步光亮镀层、细化晶粒,与DMH有协同作用。循环伏安测试研究了镀液的电化学行为,研究表明在此体系中Au³⁺的还原为两步还原过程,分别为Au³⁺→ Au⁺和Au⁺→ Au。此外DMH和胞嘧啶的添加不会带来副反应。     

基于咪唑盐离子液体固定GO_x于Au/石墨烯复合材料电极表面的葡萄糖酶传感器研究

利用长链离子液体特殊的性质,用其固定葡萄糖氧化酶(GOx)于Au/石墨烯电极表面组装成Nafion/GOx/[C10-mim+]Br-/Au/Gr修饰电极,然后用其测定葡萄糖。用透射电镜表征氧化石墨烯和Au/氧化石墨烯的形貌发现,金纳米颗粒很均匀的分散在石墨烯表面,并不存在团聚现象。电化学数据显示,Nafion/GOx/[C10-mim+]Br-/Au/Gr修饰电极对葡萄糖具有很好的催化作用,葡萄糖浓度在6.0×10-5~2×10-3mol/L范围内呈良好的线性关系(R=0.997),检出限为1.6×10-5mol/L。     

碳纳米管修饰电极上葡萄糖氧化酶的直接电子转移

制备了碳纳米管修饰玻碳电极(CNT/GC), 利用吸附的方法将葡萄糖氧化酶(GOx)固定到CNT/GC电极表面, 形成GOx-CNT/GC电极．研究了GOx的直接电子转移, 实验结果表明, GOx在CNT/GC电极表面没有发生变性, 能进行有效和稳定的直接电子转移反应, 其循环伏安图上表现出一对很好的、几乎对称的氧化还原峰; 式量电位E^0’几乎不随扫速(至少在10~140 mV·s^&#8722;1的扫速范围内)而变化, 其平均值为&#8722;0.456±0.0008 V (vs. SCE); GOx在CNT/GC电极表面直接电子转移的速率常数为1.74±0.42 s^&#8722;1, 比文献中报道的值大了数十倍; 进一步的实验结果显示, 固定在CNT/GC电极表面的GOx能保持其对葡萄糖氧化的生物电催化活性, 而且电催化活性很稳定. 文中制备碳纳米管修饰电极和固定酶的方法具有简单和易于操作等优点, 可用于获得其他生物氧化还原蛋白质和酶的直接电子转移.     

Pt nanoparticles modified Au nanowire array for amperometric and potentiometric detection of glucose

A new glucose biosensor, based on the modification of highly ordered Au nanowire arrays (ANs) with Pt nanoparticles (PtNPs) and subsequent surface adsorption of glucose oxidase (GOx), is described. Morphologies of ANs and ANs/PtNPs were observed by scanning electron microscope. The electrochemical properties of ANs, ANs/GOx, ANs/PtNPs, and ANs/PtNPs/GOx electrodes were compared by cyclic voltammetry. Results obtained from comparison of the cyclic voltammograms show that PtNPs modification enhances electrochemical catalytic activity of ANs to H₂O₂. Hence, ANs/PtNPs/GOx biosensor exhibits much better sensing to glucose than ANs/GOx. Optimum deposition time of ANs/PtNPs/GOx biosensor for both amperometric and potentiometric detection of glucose was achieved to be 150 s at deposition current of 1?×?10^?6 A. A sensitivity of 0.365 μA/mM with a linear range from 0.1 to 7 mM was achieved for amperometric detection; while for potentiometric detection the sensitivity is 33.4 mV/decade with a linear range from 0.1 to 7 mM.     

An Amperometric Glucose Biosensor Based on Poly (Pyrrole‐2‐Carboxylic Acid)/Glucose Oxidase Biocomposite

A newly developed amperometric glucose biosensor based on graphite rod (GR) working electrode modified with biocomposite consisting of poly (pyrrole‐2‐carboxylic acid) (PCPy) particles and enzyme glucose oxidase (GOx) was investigated. The PCPy particles were synthesized by chemical oxidative polymerization technique using H₂O₂ as initiator of polymerization reaction and modified covalently with the GOx (PCPy‐GOx) after activation of carboxyl groups located on the particles surface with a mixture of N‐(3‐dimethylaminopropyl)‐N′‐ethylcarbodiimide hydrochloride (EDC) and N‐hydroxysuccinimide (NHS). Then the PCPy‐GOx biocomposite was dispersed in a buffer solution containing a certain amount of bovine serum albumin (BSA). The resulting biocomposite suspension was adsorbed the on GR electrode surface with subsequent solvent airing and chemical cross‐linking of the proteins with glutaraldehyde vapour (GR/PCPy‐GOx). It was determined that the current response of the GR/PCPy‐GOx electrodes to glucose measured at +300 mV vs Cl reference electrode was influenced by the duration of the PCPy particles synthesis, pH of the GOx solution used for the PCPy particles modification and the amount of immobilized PCPy‐GOx biocomposite. An optimal pH of buffer solution for operation of the biosensor was found to be 8.0. Detection limit was determined as 0.039 mmol L⁻¹ according signal to noise ratio (S/N: 3). The proposed glucose biosensor was tested in human serum samples.     

Direct Electrochemistry of Glucose Oxidase Immobilized at a Novel Composite Material β‐Cyclodextrin/poly(4‐aminothiophenol)/Au Nanoparticle Modified Electrode

A novel complex material was fabricated by three steps. In the first step, gold nanoparticle (Au_nano) was prepared with the method of chemistry and dialysis. In the second step, 4‐aminothiophenol (AT) was encapsulated in the cavity of β‐cyclodextrin and formed inclusion complex, cyclodextrin/4‐aminothiophenol (CD/AT). And then inclusion complex was adsorbed to the surface of Au_nano based on the bond of Au‐S interaction. In the last step, a complex material, cyclodextrin/poly(4‐aminothiophenol)‐Au nanoparticles (CD/PAT‐Au_nano) was obtained by the polymerizing in the acid solution initiated by chlorauric acid. The CD/PAT‐Au_nano has spherical nanostructure with the average diameter of 55 nm. Glucose oxidase (GOx) was anchored with this complex material and direct electrochemistry of GOx was achieved. A couple of stable and well‐defined redox peaks were observed with the formal potential (E^0′) of ‐0.488 V (vs. SCE) in a pH 6.98 buffer solution. The GOx modified electrode also exhibited an excellent electrocatalytic activity to the reduction of glucose, a linearity range for determination of glucose is from 0.25 mM to 16.0 mM with a detection limit of 0.09 mM (S/N = 3). This protocol had potential application to fabricate the third‐generation biosensor.     

Avidin and Glucose Oxidase‐non‐covalently Functionalized Multi‐walled Carbon Nanotubes: A New Analytical Tool for Building a Bienzymatic Glucose Biosensor

We report an innovative supramolecular architecture for bienzymatic glucose biosensing based on the non‐covalently functionalization of multi‐walled carbon nanotubes (MWCNTs) with two proteins, glucose oxidase (GOx) (to recognize glucose) and avidin (to allow the specific anchoring of biotinylated horseradish peroxidase (b‐HRP)). The optimum functionalization was obtained by sonicating for 10 min 0.50 mg mL^?1 MWCNTs in a solution of 2.00 mg mL^?1 GOx+1.00 mg mL^?1avidin prepared in 50 : 50 v/v ethanol/water. The sensitivity to glucose for glassy carbon electrodes (GCE) modified with MWCNTs‐GOx‐avidin dispersion and b‐HRP (GCE/MWCNTs‐GOx‐avidin/b‐HRP), obtained from amperometric experiments performed at ?0.100 V in the presence of 5.0×10^?4 M hydroquinone, was (4.8±0.3) μA mM^?1 (r²=0.9986) and the detection limit was 1.2 μM. The reproducibility for 5 electrodes using the same MWCNTs/GOx‐avidin dispersion was 4.0 %, while the reproducibility for 3 different dispersions and 9 electrodes was 6.0 %. The GCE/MWCNT‐GOx‐avidin/b‐HRP was successfully used for the quantification of glucose in a pharmaceutical product and milk.     

High‐Performance Amperometric Sensors Using Catalytic Platinum Nanoparticles‐Thionine‐Multiwalled Carbon Nanotubes Nanocomposite

Thionine (TH) adsorbed on multiwalled carbon nanotubes (MWCNTs) increases the load and dispersion of platinum nanoparticles (PtNPs) generated by chemical reduction of H₂PtCl₆ with NaBH₄. Under the optimum conditions, the PtNPs‐TH‐MWCNTs/Au electrode electrocatalyzed the reduction and oxidation of H₂O₂ with high sensitivity, and after glucose oxidase (GOx) adsorption it responded to glucose concentration with a sensitivity of 0.14 A M^?1 cm^?2. The cyclic voltammetric cathodic peak current for NO₂^? reduction on PtNPs‐TH‐MWCNTs/Au responded linearly to NO₂^? concentration from 0.5 to 150 µM, with a sensitivity of 5.52 A M^?1 cm^?2 and a detection limit of 0.2 µM.     

Immobilization of glucose oxidase on rod-like and vesicle-like mesoporous silica for enhancing current responses of glucose biosensors

The use of rod-like and vesicle-like mesoporous SiO₂ particles for fabricating high performance glucose biosensors is reported. The distinctively high surface areas of mesoporous structures of SiO₂ rendered the adsorption of glucose oxidase (GOx) feasible. Both morphologies of SiO₂ enhanced the sensitivities of glucose biosensors, but by a factor of 36 for vesicle-like SiO₂ and 18 for rod-like SiO₂, respectively. The greater enhancement of vesicle-like SiO₂ can be accounted for by its higher specific surface area (509 m² g⁻¹) and larger total pore volume (1.49 cm³ g⁻¹). Interestingly, the current responses of GOx immobilized in interior channels of the mesoporous SiO₂ were enhanced much more than those of simple mixtures of GOx and the mesoporous SiO₂. This suggests that the enhancement of current responses arise not only from the high surface area of SiO₂ for high enzyme loading, but also from the improved enzyme activity upon its adsorption on mesoporous SiO₂. Also compared were the performances of glucose biosensors with GOx immobilized on mesoporous SiO₂ by physical adsorption and by covalent binding to 3-aminopropyltrimethoxysilane (APTMS) modified SiO₂ using glutaraldehyde as the cross-linker. The covalent binding approach resulted in higher enzyme loading but lower current sensitivity than with the physical adsorption.     

Incorporation of glucose oxidase into Langmuir-Blodgett films based on Prussian blue applied to amperometric glucose biosensor

Glucose oxidase (GOx) was immobilized in the organic-inorganic Langmuir-Bldogett (LB) films consisting of octadecyltrimethylammonium (ODTA) and nanosized Prussian blue (PB) clusters. The amperometric glucose biosensors based on the LB films were fabricated and tested. It was found that the sensors exhibited a clear response current under an applied voltage of 0.0 V (vs Ag/AgCl). The linearity of current density versus glucose concentration was confirmed below 15 mmol/L concentration. This is the first observation of biosensor function of the hybrid organic-inorganic LB films. The successful preparation of glucose sensors operating at the very low potential indicates that the adsorbed PB clusters in the LB films act as an electrocatalyst for the electrochemical reduction of hydrogen peroxide, which is the final product of the enzymatic reaction sequence. The observed low potential applicability is estimated to inhibit the responses of interferants such as ascorbic acid, uric acid, and acetominophen. It was also found that an electrostatic interaction between positively charged ODTA+ and the adsorbed species of both GOx and PB provided a stabilized adsorption state in the LB films. Such stable immobilization contributes to the steady amperometric response current observed in the present ODTA/PB/GOx LB films.     

Glucose biosensor based on graphite electrodes modified with glucose oxidase and colloidal gold nanoparticles

The electrochemistry of glucose oxidase (GOx) immobilized on a graphite rod electrode modified by gold nanoparticles (Au-NPs) was studied. Two types of amperometric glucose sensors based on GOx immobilized and Au-NPs modified working electrode (Au-NPs/GOx/graphite and GOx/Au-NPs/graphite) were designed and tested in the presence and the absence of N-methylphenazonium methyl sulphate in different buffers. Results were compared to those obtained with similar electrodes not containing Au-NPs (GOx/graphite). This study shows that the application of Au-NPs increases the rate of mediated electron transfer. Major analytical characteristics of the amperometric biosensor based on GOx and 13 nm diameter Au-NPs were determined. The analytical signal was linearly related to glucose concentration in the range from 0.1 to 10 mmol L^?1. The detection limit for glucose was found within 0.1 mmol L^?1 and 0.08 mmol L^?1 and the relative standard deviation in the range of 0.1–100 mol L^?1 was 0.04–0.39%. The τ_1/2 of V _max characterizes the storage stability of sensors: this parameter for the developed GOx/graphite electrode was 49.3 days and for GOx/Au-NPs/graphite electrode was 19.5 days. The sensor might be suitable for determination of glucose in beverages and/or in food.     

Direct electrochemical sensing of glucose using glucose oxidase immobilized on functionalized carbon nanotubes via a novel metal chelate-based affinity method

We report on a novel amperometric glassy carbon biosensing electrode for glucose. It is based on the immobilization of a highly sensitive glucose oxidase (GOx) by affinity interaction on carbon nanotubes (CNTs) functionalized with iminodiacetic acid and metal chelates. The new technique for immobilization is exploiting the affinity of Co(II) ions to the histidine and cysteine moieties on the surface of GOx. The direct electrochemistry of immobilized GOx revealed that the functionalized CNTs greatly improve the direct electron transfer between GOx and the surface of the electrode to give a pair of well-defined and almost reversible redox peaks and undergoes fast heterogeneous electron transfer with a rate constant (k _s) of 0.59?s^?1. The GOx immobilized in this way fully retained its activity for the oxidation of glucose. The resulting biosensor is capable of detecting glucose at levels as low as 0.01?mM, and has excellent operational stability (with no decrease in the activity of enzyme over a 10?days period). The method of immobilizing GOx is easy and also provides a model technique for potential use with other redox enzymes and proteins.

Electrocatalytic Activity of Nanohybrids Based on Carbon Nanomaterials and MFe2O4 (M=Co,Mn) towards the Reduction of Hydrogen Peroxide

We report the advantages of hybrid nanomaterials prepared with electrogenerated ferrites (MFe₂O₄; M: Co, Mn) and multi‐walled carbon nanotubes (MWCNTs) or thermally reduced graphene oxide (TRGO) on the electro‐reduction of hydrogen peroxide. Glassy carbon electrodes (GCE) modified with these hybrid nanomaterials dispersed in Nafion/isopropanol demonstrated a clear synergism on the catalytic reduction of reduction of hydrogen peroxide at pH 13.00. The intimate interaction between MFe₂O₄ and carbon nanomaterials allowed a better electronic transfer and a facilitated regeneration of M²⁺ at the carbon nanomaterials, reducing the charge transfer resistances for hydrogen peroxide reduction and increasing the sensitivities of the amperometric response.