壳聚糖固定化葡萄糖氧化酶生物传感器测定葡萄糖的含量

应用壳聚糖将葡萄糖氧化酶固定于鸡蛋膜上,结合氧电极制得葡萄糖传感器.实验表明,壳聚糖比戊二醛能更好地固定葡萄糖氧化酶,最佳条件为壳聚糖浓度0.3%、固定化酶量0.8 mg、 pH 7.0、缓冲溶液浓度300 mmol/L和温度25 ℃.本葡萄糖传感器的线性范围为0.016～1.10 mmol/L;检出限为8.0 μmol/L(S/N=3), 响应时间<60 s,有很好的稳定性,寿命>3个月.同一个传感器重复使用以及同方法制作的不同传感器之间都有很好的重现性,RSD分别为2.5%(n=10)和4.7%(n=4).实际样品中可能存在的烟酰胺、 VB6、 VB12、 VE、Ca2+、 Mg2+、 K+和Zn2+等对葡萄糖的测定不产生干扰.本传感器已成功地应用于市售饮料中葡萄糖含量的测定.     

葡萄糖基-β-环糊精作为手性选择剂对苯磺酸氨氯地平的毛细管电泳手性拆分

以葡萄糖基-β-环糊精(Glu-β-CD)为手性选择剂,用毛细管区带电泳法对手性药物苯磺酸氨氯地平进行了拆分研究.考察了缓冲液的pH值、缓冲液浓度、缓冲液体系组成、Glu-β-CD的浓度及电压等对分离的影响,并对3批市售左旋苯磺酸氨氯地平片(施慧达)进行光学纯度检查.结果表明,在背景电解质为含20 mmol/L Glu-β-CD的200 mmol/L乙酸-三乙醇胺(HAc-TEA)(pH 4.0)体系,电压25 kV,温度20 ℃,检测波长214 nm的条件下,苯磺酸氨氯地平可以得到良好分离,分离度为4.0.     

硅溶胶-凝胶包埋纳米金和酶的葡萄糖生物传感器

采用溶胶-凝胶技术将金纳米粒子和葡萄糖氧化酶一次性固定于硅溶胶-凝胶的网络结构中,制备了葡萄糖生物电化学传感器并优化了传感器的制备条件。酶电极对葡萄糖具有良好的电化学响应,葡萄糖浓度在0.02~2.0 mmol/L范围内和催化电流呈线性关系,检出限为0.005 mmol/L。酶电极在4 ℃下贮存100 d后对葡萄糖的响应仅下降8%。该酶电极灵敏度高、响应快、稳定性好。     

利用层层累积技术制备基于纳米碳管的葡萄糖生物传感器

以多壁纳米碳管(MWNTS)为电子媒介体和酶的吸附载体,利用层层累积的自组装技术固定葡萄糖氧化酶(GOX)的多层(MWNTa/GOx).复合薄膜修饰电极,制备了一种新型葡萄糖生物传感器.结果表明,传感器对葡萄糖的响应电流值随着MWNTa//GOx复合薄膜层数的不同而变化,当MWNTa//GOx复合薄膜的层教为6时,响应电流值迭到最大.(MWNTs/GOx).复合薄膜修饰的葡萄糖生物传感器对30mmol/L葡萄糖的响应电流为1.63μA,响应时间仅为6.7 s.该生物传感器检测的线性范围为0.5～15 mmol/L,最低检测浓度可达0.09 mmol/L.     

普鲁士蓝修饰电极结合硅溶胶-凝胶技术制备高灵敏葡萄糖传感器

基于普鲁士蓝修饰玻碳电极结合二氧化硅溶胶 凝胶固定化酶技术构造具有“三明治”式结构的酶电极。考察了酶电极对葡萄糖的电化学响应以及操作条件。结果表明 :所制备的传感器在pH 6 .5 ,电位为- 0 .0 5V条件下对葡萄糖在 0～ 5mmol/L呈线性响应 ,响应时间为 12s ,检出限为 0 .0 2mmol/L ,灵敏度高达1 182 μA/ (mmol·L-1)。传感器的稳定性好 ,4 5d其响应值仍保持 90 %。     

蛇床子及其制剂中香豆素类活性成份的胶束电动毛细管色谱含量测定

建立了胶束电动毛细管色谱分离和测定蛇床子及其制剂中3种香豆素类活性组分的方法.系统考察了背景电解质pH、表面活性剂浓度、有机改性剂种类和浓度对分离的影响.实验结果表明:在缓冲液浓度为10 mmol/L、缓冲液pH为10.5、SDS浓度为20 mmol/L、甲醇浓度为10%时的优化条件下,蛇床子及其制剂中3种香豆素类活性组分得到基线分离.且方法具有较好的重现性.     

基于金纳米棒-壳聚糖复合膜的葡萄糖生物传感器

本文采用金纳米棒-壳聚糖复合膜固定葡萄糖氧化酶构建电流型葡萄糖生物传感器.通过电化学交流阻抗法和循环伏安法对酶膜状态进行了表征,得到了相应的等效电路和动力学参数.实验结果表明,金纳米棒-壳聚糖复合膜可以辅助电子传递,提高电极的电流响应,并使生物传感器的使用温度范围有很大的扩展.此传感器表现出对葡萄糖溶液浓度的优良响应,线性范围在2.78×10^-5mol/L—2.22×10^-3mol/L,响应灵敏度约为7.819μA·cm^-2(mmol/L)^-1,表观米氏常数为10mmol/L.本工作还研究了温度和溶液pH值对电极电流响应的影响.     

水溶性量子点碲化镉测定同型半胱氨酸的研究

以巯基丙酸为稳定剂,在水溶液中一步合成了CdTe量子点,以该量子点为荧光探针,基于荧光增敏法对同型半胱氨酸(Hcy)进行选择性测定,考察了缓冲体系、缓冲液浓度、缓冲液pH值、反应时间、量子点浓度等多种因素的影响.在0.05 mol/L、pH 8.8的磷酸二氢钠-磷酸氢二钠缓冲液中,当量子点浓度为1.2 mmol/L、反应时间为10 min时,该方法的线性区间为0.1 ～60 μmol/L,检出限为8×10-8 mol/L.     

基于纳米复合材料/壳聚糖膜的葡萄糖生物传感器研究

采用纳米普鲁士蓝/金纳米粒子/壳聚糖(nano-PB/AuNPs/Chit)复合膜固定葡萄糖氧化酶(GOD)构建新型葡萄糖生物传感器。通过电化学阻抗谱以及电流-时间曲线法(I-t)研究了传感器的电化学特性。结果表明,传感器在葡萄糖浓度为0.01～1.0 mmol/L范围内呈线性,响应灵敏度为68.15μA.(mmol/L)-1.cm-2,表观米氏常数为5.1 mmol/L。该传感器可用于糖尿病人血糖的测定。     

电堆积在线扫集胶束电动色谱法测定苦参中的生物碱

建立了电堆积在线扫集胶束电动色谱法测定苦参碱和槐定碱的新方法.考察了pH值、磷酸二氢钠浓度、CTAB浓度、电压、有机溶剂和进样时间对分离效果的影响.采用未涂层熔融石英毛细管,以20mmol/L磷酸二氢钠-0.8 mmol/L CTAB-100mmol/L Tris(含10%异丙醇,pH 8.9)为缓冲液,在进样电压-1...     

纳米金-还原氧化石墨烯修饰葡萄糖氧化酶传感器的制备及其电流法检测饮料中的葡萄糖

利用纳米金(Au NPs)与还原氧化石墨烯(rGO)复合纳米材料制备了葡萄糖氧化酶生物传感器并用于饮料中葡萄糖含量的检测。将壳聚糖作为还原剂及稳定剂,通过一步法合成了Au NPs-rGO复合材料,并通过物理吸附固定葡萄糖氧化酶(GOx)来制作GOx生物传感器。该传感器在磷酸盐缓冲溶液(0.1 mol/L,p H6.0)中,-0.45 V(vs.Ag/Ag Cl)电位下电流法检测葡萄糖含量,线性检测范围为0.01~0.88 mmol/L,灵敏度为22.54μA·mmol-1·L·cm-2,检出限为1.01μmol/L,且表观米氏常数为0.497 mmol/L。该传感器用于多种饮料中葡萄糖含量的直接检测,结果满意。     

A Microdialysis Probe Coupled with A Miniaturized Thermal Glucose Sensor for In Vivo Monitoring

Abstract

A miniaturized thermal flow injection analysis biosensor has been coupled with a microdialysis probe for continuous subcutaneous glucose monitoring. Thermal biosensors are based on the principle of measuring the heat evolved during enzyme catalysed reactions. The system presented here consists of a miniaturized thermal biosensor with a small column containing coimmibolized glucose oxidase and catalase. The analysis buffer passes through the column at a flow rate of 60μL/min via an 1μL sample loop which is connected to a microdialysis probe.

Invitro results showed constant permeability of the probe and stability of the biosensor response during 24 hours. The response time was 85 sec giving a sample rate of 42 samples/hour.

During a load experiment, the glucose profile in a healthy volunteer was followed both in the subcutaneous tissue and blood using the microdialysis set-up proposed and comparing to blood glucose analyser.     

Glucose Biosensor Using Glucose Oxidase Immobilized in Polyaniline

A biosensor for glucose utilizing kinetics of glucose oxidase (EC 1.1.3.4.) was developed. The enzyme was immobilized on polyaniline by covalent bonding, using glutaraldehyde as a bifunctional agent. The system showed a linear response up to 2.2 mM of glucose with a response time of 2.5–4.0 min. In addition, the immobilized enzyme had a higher activity between pH 6.5 and 7.5. The system retained 50% of its activity after 30 d of daily use. The optical absorption spectra of the polyaniline/glucose oxidase electrode after glucose had been added to the buffer solution showed that the absorption band around 800 nm had changed considerably when glucose was allowed to react with the electrode. This optical variation makes polyaniline a very promising polymer for use as a support in optical sensor for clinical application.     

Improved biosensor for glucose based on glucose oxidase-immobilized silk fibroin membrane

Based on glucose oxidase-immobilized silk fibroin membrane and oxygen electrode, the authors have developed an amperometric glucose sensor in flow-injection analysis. After the sensor was improved by the configuration of oxygen electrode and a temperature control system was added to the electrode body, its sensitivity, analytical precision, and stability were enhanced greatly. The authors first introduced a tailing inhibitor-ion pair reagent into a buffer system in the biosensor so as to eliminate all interference from hemacyte, macromolecules, and small mol wt charged species besides electroactive specie ascorbate in complex matrices. A considerably serious tailing of the biosamples, such as whole blood, plasma, serum, or urine on the sensor, based on enzyme electrode, entirely disappeared, their response times were shortened, and base lines became more smooth and stable. The glucose sensor has a broad range of linear response for glucose (up to 25.0 mmol/L) and a good correlation (γ = 0.999) under conditions of control temperature 32.0°C and 1.6 mL/min 0.02 mol/L phosphate buffer containing 0.5% tailing inhibitor (v/v). Recoveries of glucose in these biosamples are within the range of 93.71–105.88%, and its repeatabilities for determining glucose, repeated 100 times, human blood dilution 125 times, and serum 128 times, are 1.81,2.48, and 2.91% (RSD), respectively. The correlation analysis for 200 serum samples showed that the correlation (γ) is 0.9934 between the glucose sensor and Worthington method for determining serum glucose used conventionally in a hospital laboratory. Moreover, the enzyme membrane used in the biosensor can be stored for a long time (over 2 yr) and measured repeatedly over 1000 times for biosamples. The glucose sensor is capable of detecting over 60 biosamples/hr.     

Thin-film biosensor for the measurement of glucose concentration in human serum and urine

Solid-state technology and pulse electroplating were used to fabricate a glucose biosensor based on hydrogen peroxide detection. This glucose biosensor was composed of thin-film electrodes, and enzyme-immobilized and deactivated enzyme-immobilized membranes. The electrodes were fabricated by metallic film deposition. Cr and Ni adhesive layers were applied successively by vapour deposition on the thermally oxidized SiO₂ isolating layer on a silicon substrate, and then the two metallic layers were patterned by the photolithographic method. Subsequently, a 1 μm thick Au layer was applied by means of pulse electroplating, forming two anodes and one common cathode in each sensor chip. On one anode, glucose oxidase (GOD) was immobilized by cross-linking with bovin serum albumin and glutaraldehyde. A deactivated GOD-immobilized membrane was formed on the other anode, which worked as a reference working electrode. A novel differential measurement system was used to treat the output signals of the two anodes by adjusting the initial position of the response curves, compensating amplifications of the individual I—V converters and treating the output signals with a subtraction circuit in order to decrease measurement error. The test results showed that the signal of ascorbic acid up to 4.5 mmol 1⁻¹ or uric acid up to 1.2 mmol 1⁻¹ was successfully cancelled. Glucose concentrations in the range 0.02–4.0 mmol/1 could be detected and an excellent linear response was obtained in the low concentration range. The correlation coefficient between the result of the enzyme electrode and the clinically enzymatic method for glucose measurement in human serum was 0.9912. Correlated results between the biosensor method and the routine clinical method for the measurement of glucose concentration in urine were obtained. The lifetime of the enzyme electrode was over 2 months.     

Organically Modified Sol‐Gel/Chitosan Composite Based Glucose Biosensor

A new type of organically modified sol‐gel/chitosan composite material was developed and used for the construction of glucose biosensor. This material provided good biocompatibility and the stabilizing microenvironment around the enzyme. Ferrocene was immobilized on the surface of glassy carbon electrode as a mediator. The characteristics of the biosensor were studied by cyclic voltammetry and chronoamperometry. The effects of enzyme‐loading, buffer pH, applied potential and several interferences on the response of the enzyme electrode were investigated. The simple and low‐cost glucose biosensor exhibited high sensitivity and good stability.     

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.     

Fast and Effective Turn‐on Paper‐based Phosphorescence Biosensor for Detection of Glucose in Serum

In this study, a turn‐on paper‐based optical analytical system with a rapid, sensitive and quantitative response for glucose was developed. The luminescence sensing material, crystalline iridium(III)‐Zn(II) coordination polymers, or Ir‐Zn_e, was grown electrochemically on stainless steel mesh and then deposited on filter paper. This sensing substrate was subsequently built up under glucose oxidase encapsulated in hydrogel and then immobilized on egg membrane with the layer‐by‐layer method. Once the glucose solution was dropped onto the paper, the oxygen content was depleted simultaneously with a concomitant increase in the phosphorescence of Ir‐Zn_e. The detection limit for glucose was 0.05 mM. The linear dynamic range for the determination of glucose was 0.05–8.0 mM with a correlation coefficient (R²) of 0.9956 (y=68.11 [glucose]?14.72). The response time was about 0.12 s, and the sample volume was less than 5 μL. The effects of mesh size, buffer concentration, pH, enzyme concentration, temperature, and interference, and the stability of the biosensor, have also been studied in detail. Finally, the biosensor was successfully applied to the determination of glucose in human serum.     

基于Dy_2(MoO_4)_3-AuNPs复合纳米材料的葡萄糖生物传感器

采用水热法合成了纳米材料钼酸镝[Dy_2(MoO_4)_3],并制备了Dy_2(MoO_4)_3-AuNPs复合材料,利用该复合材料固定葡萄糖氧化酶(GOD)构建了葡萄糖生物传感器.通过透射电子显微镜(TEM)、紫外-可见光谱(UV-Vis)和能谱分析(EDS)等手段对所制备的材料进行了表征,并利用电化学阻抗谱(EIS)和循环伏安(CV)曲线研究了该传感器的电化学性能.结果表明,Dy_2(MoO_4)_3-AuNPs复合材料具有较好的生物相容性,能增强固定化的GOD的生物活性,并促进GOD在电极表面的电子传递速率;该传感器在葡萄糖浓度为0.01~1.0 mmol/L范围内葡萄糖浓度与响应电流呈较好的线性关系,最低检出限为3.33μmol/L(S/N=3),该生物传感器还具有较好的稳定性和重现性.