基于树枝状分子及功能化金纳米粒子的电化学免疫传感器检测污泥中大肠杆菌

利用树枝状分子-金纳米粒子复合物修饰电极和金纳米粒子标记物构建电化学免疫传感器,用于污泥中大肠杆菌的检测.首先在玻碳电极表面电聚合对氨基苯甲酸,通过共价作用结合第Ⅳ代氨基末端的树枝状分子(G4-PAMAM),并在其内部载入金纳米粒子,制备修饰电极(GCE/p-ABA/PAMAM (AuNPs)),用于固定大肠杆菌.采用硫堇作为电活性物质包被金纳米粒子,用于标记二抗制备金纳米粒子标记物(Ab2-Au-Th).通过抗原-抗体之间的特异性识别作用,将一抗、金纳米粒子标记物依次修饰在电极表面,用差分脉冲伏安法测定硫堇产生的电流信号,实现对大肠杆菌的检测.在优化的实验条件下,响应电流与大肠杆菌浓度的对数在1.0×102～1.0×106 cfu/mL范围内呈线性关系,检出限为70 cfu/mL(S/N=3).利用本方法检测污水处理厂的不同污泥样品中的大肠杆菌,回收率为89.4％～ 105.8％.     

基于碳纳米管固定抗原的电化学免疫传感器法测定IgG抗体

以1-萘酚磷酸酯为底物,将IgG抗原吸附固定在碳纳米管修饰玻碳电极的表面,利用待测IgG抗体和碱性磷酸酯酶标记IgG抗体共同竞争免疫传感器表面的IgG抗原,研制了一种新型的电化学免疫传感器用于IgG抗体的测定。碱性磷酸酯酶可以催化底物1-萘酚磷酸酯水解生成1-萘酚,在电极表面氧化产生电信号。在电位为+0.30 V(vs.SCE)时,响应电流与IgG抗体浓度在5.0×10-9～5.0×10-7g/mL范围内呈良好的线性关系,检出限为2.0×10-9g/mL。     

基于免疫胶体金试纸条检测盐酸克伦特罗的便携式光电型传感器

利用免疫竞争抗制原理制备检测盐酸克伦特罗的免疫纳米金试纸条,盐酸克伦特罗与CLB-BSA复合物竞争性结合胶体金上抗体的有限位点,从而使试纸条上的检测带显色减弱或消失.将显色后的试纸条插入自行研制的光电型传感器的测试孔内,根据反射光的强弱计算出克伦特罗的浓度.结果表明:用光电传感方法检测盐酸克伦特罗的线性范围为1～10 μg/L,检出限为0.05 μg/L,回收率为85.5％～96.0％.此光电型传感器检测克伦特罗具有简便、快速、灵敏、特异性强的优点.     

基于蛋白A/纳米金/壳聚糖分散的多壁碳纳米管修饰的电位型甲胎蛋白免疫传感器的研究

将壳聚糖分散的多壁碳纳米管(MWNT-CS)滴涂于金电极(Au)表面,利用壳聚糖大量的氨基将纳米金(nano-Au)固定到金电极表面,再利用蛋白A(PA)的定向固定效应将甲胎蛋白抗体(anti-AFP)固定到纳米金修饰的金电极表面,从而制得高灵敏、高稳定电位型甲胎蛋白免疫传感器。蛋白A为抗原和抗体的反应提供了合理的基础,纳米金的存在提高了抗体在电极表面的固定量,多壁碳纳米管(MWNT)促进了电子的传递,从而缩短电极的响应时间。在优化的实验条件下,该传感器响应的电极电位与甲胎蛋白浓度的对数在7.0~190.0μg/L的范围内保持良好的线性关系,检出限(S/N=3)为3.9μg/L。     

基于Ru@SiO_2的微囊藻毒素电化学发光免疫传感器研究

本研究在玻碳电极(GCE)表面电沉积金纳米粒子(Au NPs),通过化学吸附将微囊藻毒素-(亮氨酸-精氨酸)(MC-LR)的单克隆抗体(anti-MC-LR)固定在电沉积了Au NPs的玻碳电极表面,以牛血清白蛋白(BSA)封闭非特异性吸附位点,制得免疫电极anti-MC-LR/Au NPs/GCE。采用微乳化法制备了掺杂三(2,2'-联二吡啶)钌(Ⅱ)配合物离子(Ru(bpy)2+3)的二氧化硅纳米粒子(Ru@SiO2),利用透射电镜和扫描电镜对所制备的纳米粒子进行表征。3-氨基丙基三乙氧基硅烷(APTS)进一步与Ru@SiO2反应,制得氨基功能化的Ru@SiO2,通过1-(3-二甲氨基丙基)-3-乙基碳二亚胺(EDC)和N-羟基琥珀酰亚胺(NHS)活化辣根过氧化物酶标记的MC-LR(HRP-MC-LR),并使其与氨基功能化的Ru@SiO2偶联,制得MC-LR-Ru@SiO2。采用直接竞争模式,在标记物MC-LR-Ru@SiO2存在下,以三丙胺作为共反应物,利用电化学发光法(ECL)测定溶液中的微囊藻毒素,免疫反应完成后,电化学发光强度(I)随着MC-LR浓度的增大而减小,且在0.100~100μg/L范围内,电化学发光强度差值(ΔI)与游离的MC-LR浓度的对数呈良好线性关系,检出限为0.007μg/L。对实际水样进行了加标回收实验,回收率为95.5%~105%。     

纳米金/丝素复合膜修饰电极制备及对对苯二酚的电催化作用

将丝素还原HAuCl4制备的纳米金/丝素溶胶修饰在金电极表面制备了纳米金/丝素复合膜修饰电极,用于对苯二酚的催化氧化。实验表明,该修饰电极具有很好的电化学性能,在pH3.55磷酸盐缓冲溶液中以该修饰电极对对苯二酚进行检测,对苯二酚在4.0×10-6~1.0×10-4mol/L浓度范围内,其氧化峰电流与浓度呈良好的线性关系,其线性回归方程为i(μA)=0.2614 5.3539c,r=0.9995;检出限为2.0×10-7mol/L,灵敏度良好,用于实际样品分析,结果令人满意。     

纳米二氧化钛-氧化锌/硅溶胶/导电胶复合材料固定联吡啶钌制备磷酸可待因电化学发光传感器

利用硅溶胶的成膜性、纳米二氧化钛-氧化锌大的比表面积及导电胶的粘结性,制备了纳米二氧化钛-氧化锌/硅溶胶/导电胶复合材料,基于此复合材料将联吡啶钌固定到金电极表面,制备了磷酸可待因电化学发光(ECL)传感器.在优化的实验条件(800 V负高压、扫描速度100 mV/s,磷酸盐缓冲体系(pH 6.5))下,可待因浓度在1.0×10-7～1.0×10-4 mol/L范围内与电化学发光强度呈良好的线性关系(r2=0.9973),检出限为2.56×10-8 mol/L (S/N=3).传感器表现出良好的重现性与稳定性,连续平行测定1.28×10-5 mol/L可待因溶液10次,发光强度的相对标准偏差(RSD)为2.7％;室温下保存10天后,发光强度为初始值的92％以上.测定可待因药物实际样品的加标回收率在99.3％ ～ 102.5％之间.     

免标记电化学免疫传感器用于微囊藻毒素-LR的灵敏检测

采用纳米金作为抗体的固定基质,同时以硫堇为电活性指示剂,构建了一种免标记的电化学免疫传感器用于微囊藻毒素-LR(MC-LR)的灵敏检测。将萘酚修饰到金电极表面,通过静电作用将硫堇捕获。加入纳米金与硫堇的氨基结合,抗体将通过与纳米金作用而固定到电极表面。通过MC-LR与其相应抗体的特异性结合作用阻碍硫堇的电子传递,实现MC-LR的电化学检测。在最优实验条件下,MC-LR的质量浓度与电信号在5~100μg/L范围内呈良好的线性关系,检出限为0.71μg/L,可满足饮用水检测需求,能够用于实际水样中M C-LR的测定。     

纳米复合物修饰电极的电化学传感器检测芦丁

研制了纳米复合物修饰电极,碳纳米管与表面含有大量氨基的壳聚糖在玻碳电极表面首先形成碳纳米管/壳聚糖膜,通过膜表面丰富的氨基与纳米Au的强静电吸附,在玻碳电极表面获得均匀致密的纳米金修饰层.这种基于纳米复合材料制备的新型电化学传感器对芦丁具有很好的响应,可以快速地实现电极与芦丁之间的直接电子转移,有良好的稳定性.芦丁的测定线性范围为4.00×10-7～1.77×10-5 mol/L,最低检测限为1.29×10-7 mol/L.由于抗坏血酸在该修饰电极上的氧化电位出现显著负移,因此可避免抗坏血酸对芦丁测定的干扰.该方法可以不经预分离直接检测药物中的芦丁含量.     

基于多边形金纳米颗粒的非标记型可卡因适体传感器的研制

实验合成了多边形金纳米颗粒,通过壳聚糖(CHIT)将合成的多边形金纳米颗粒固定在玻碳电极表面,然后通过自组装技术将带巯基的捕获DNA探针固定在修饰有多边形金纳米颗粒的电极表面,利用杂交反应使可卡因适体与DNA捕获探针结合,制成非标记型可卡因适体传感器。以六氨合钌作为电化学指示剂,通过测量传感器与目标物可卡因结合前后电流变化情况对可卡因进行测定。考察了缓冲溶液的pH、可卡因培育时间、扫描速度等对测定的影响。结果表明,在pH为7.40时该传感器的检测范围为1.0×10-10～1.0×10-3 mol/L,检测限为3.0×10-11 mol/L。该传感器制作简单,响应好,抗干扰能力强。     

Determination of β-adrenergic agonists by hapten microarray

The use of highly active β-agonists as growth promoters is not appropriate because of the potential hazard for human and animal health. To investigate the residue level of these β-agonists, hapten microarrays were employed for clenbuterol (CLB), ractopamine (RAC) and salbutamol (SAL) residue analysis. CLB, RAC and SAL conjugates were immobilized on the slides, which were precoated by agarose film to construct hapten microarrays, and then the corresponding monoclonal antibodies of these β-agonists and the standards or samples were introduced for indirect competitive immunoassay. Finally, Cy3-labeled secondary antibody was employed to indicate the antigen-antibody complex. The fluorescence intensity of each spot was imaged and recorded, and the calibration curve of each analyte was obtained by plot fluorescence intensity against different standard concentrations. Compared to the ELISA, the hapten microarray method was more sensitive, which got the detection limits 0.09 μg/L for CLB, 0.50 μg/L for RAC, and 0.01 μg/L for SAL. What's more, with the recovery rate between 96.5% and 106.4%, and the coefficient of variation below 10%, the proposed hapten microarray method was shown to be both quantitative and reproducible.     

盐酸克伦特罗在乙炔黑电极上的电化学行为及其分析测定研究

研究了盐酸克伦特罗(CLB)在乙炔黑电极上的电化学行为,发现阴离子表面活性剂十二烷基苯磺酸钠(SDBS)能显著提高CLB的氧化峰电流并降低其氧化过电位。优化了实验参数,建立了一种直接测定CLB的新电分析方法,其线性范围为1.0×10-7~7.5×10-5mol/L,开路富集1 min后的检出限为2.5×10-8mol/L。平行10次测定1.0×10-5mol/L盐酸克伦特的RSD为3.1%。方法用于猪尿中盐酸克伦特罗含量的测定。     

Ultrasensitive electrochemical immunoassay based on graphene oxide-Ag composites for rapid determination of clenbuterol

We report the development of an ultrasensitive amperometric biosensor based on Ag nanoparticles-decorated graphene oxide nanosheets (GO) (Ag-GO) for the rapid detection of clenbuterol (CLB). The morphology and structure of the Ag-GO labeled CLB (Ag-GO-CLB) were characterized by transmission electron microscope (TEM), atomic force microscope (AFM), and ultraviolet-visible spectroscope (UV-vis). The immunosensor was prepared by covalently immobilizing capture antibodies on a multi-walled carbon nanotubes-modified glassy carbon electrode. Through competitive immunoreactions, the Ag-GO-CLB nanocomposites were captured on the immunosensor and the silver was measured by positive differential pulse voltammetry (DPV) in KCl solution for the detection of antigen. The experimental results show a linear response over the range from 0.01 to 10.0 ng mL(-1) with a lower detection limit of 6.8 pg mL(-1) (signal-to-noise ratio of 3). The Ag-GO based immunosensor offers a simple and convenient route for metal-immunoassay labels, which can avoid the complicated and time-consuming dissolving of metal component for ultrasensitive determination. Moreover, the electrochemical immunoassay shows acceptable specificity and stability and is suitable for the determination of CLB in real samples.     

Label-free Microcantilever Immunosensor Based on a Competitive Immunoassay for the Determination of Clenbuterol

A label-free microcantilever immunosensor based on a competitive immunoassay is reported for the determination of clenbuterol. The immunosensor was fabricated by modifying clenbuterol–ovalbumin on the gold surface of the microcantilever with crossing linkage by L-cysteine and glutaraldehyde. Atomic force microscopy was utilized to characterize the construction of immunosensor and to measure the deflection of the microcantilever. The deflection response of the microcantilever was in negatively proportional to the concentration of clenbuterol from 1.0?×?10^?2 to 20?µg/L with a limit of detection of 1.0?×?10^?2?µg/L. The fabricated immunosensor was used to determine clenbuterol in pork samples with satisfactory results. In addition, the results were in accordance with those obtained by high-performance liquid chromatography. The reported immunosensor displayed high sensitivity and specificity together with excellent repeatability and reliability.     

Electrochemical immunoassay for α-fetoprotein through a phenylboronic acid monolayer on gold

A novel reusable electrochemical immunosensor for α-fetoprotein (AFP) based on phenylboronic acid monolayer on gold was proposed. The sensor was fabricated by immobilizing of 3-aminophenylboronic acid (APBA) conjugated thiol-mixed monolayer on gold through 2-(5-norbornene-2,3-dicarboximido)-1,1,3,3-tetramethyluronium tetrafluoroborate (TNTU) as linkage. AFP and enzyme-conjugated antibody were further trapped to the modified electrode surface through sugar-boronic acid and immunoaffinity interactions, respectively. The attached enzyme-conjugated antibody on the electrode surface could catalyze the reduction of hydrogen peroxide in the presence of thionine, which can be used to detect AFP in human serum by a competitive mechanism. Cyclic voltammetric, electrochemical impedance studies and photometric activity assays were used to probe the assembly and regeneration process of the immunosensor. The influences of the competitive ratio of antigen and antibody, pH value of the measuring solution, incubation temperature and time were explored for optimizing the analytical performance. The whole assay process including incubation, detection and regeneration of the electrode could be completed in 35 min. The detection of AFP in five serum samples provided from clinically diagnosed patients with liver cancer showed acceptable accuracy. The proposed immunosensor enabled fast, low-cost and would be valuable for clinical diagnosis.     

维生素B6在纳米金/石墨烯修饰电极上的电化学行为

将金纳米粒子电沉积在石墨烯修饰的玻碳电极表面,研究了维生素B6(VB6)在该修饰电极上的电化学行为。扫描电镜用于该修饰电极组装过程的形貌表征。实验结果表明:VB6在此修饰电极上出现一个良好的氧化峰,在最佳实验条件下,其氧化峰电流与VB6浓度在5.0×10-8～2.0×10-5 mol/L范围内呈线性关系,其线性回归方程为I(μA)=0.5697c(μmol/L)+0.06275,R=0.9992,检出限为2.0×10-8 mol/L(S/N=3)。一些常见的干扰物质如抗坏血酸不干扰VB6的检测。方法已用于片剂中VB6的含量的检测。     

Amplified inhibition of the electrochemical signal of ferrocene by enzyme-functionalized graphene oxide nanoprobe for ultrasensitive immunoassay

A nanoprobe-induced signal inhibition mechanism was designed for ultrasensitive electrochemical immunoassay at a chitosan-ferrocene (CS-Fc) based immunosensor. The nanoprobe was prepared by covalently loading signal antibody and high-content horseradish peroxidase (HRP) on the graphene oxide (GO) nanocarrier. The immunosensor was prepared through the stepwise assembly of gold nanoparticles (Au NPs) and capture antibody at a CS-Fc modified electrode. After sandwich immunoreaction, the GO-HRP nanoprobes were quantitatively captured onto the immunosensor surface and thus induced the production of a layer of insoluble film through the enzymatically catalytic reaction of the HRP labels. Both the dielectric immunocomplex formed on the immunosensor surface and the enzymatic precipitate with low electroconductivity led to the electrochemical signal decease of the Fc indicator, which was greatly amplified by the multi-enzyme signal amplification of the nanoprobe. Based on this amplified signal inhibition mechanism, a new ultrasensitive electrochemical immunoassay method was developed. Using carcinoembryonic antigen as a model analyte, this method showed a wide linear range over 5 orders of magnitude with a detection limit down to 0.54 pg/mL. Besides, the immunosensor showed good specificity, acceptable reproducibility and stability as well as satisfactory reliability for the serum sample analysis.     

多壁碳纳米管-分子印迹传感器测定盐酸克伦特罗

结合碳纳米材料和分子印迹技术,建立了以K3[Fe(CN)6]为探针测定盐酸克伦特罗的方法。以邻苯二胺为功能单体,盐酸克伦特罗为模板,采用电化学聚合法在多壁碳纳米管修饰电极表面制备了分子印迹薄膜。用乙腈水溶液可快速去除模板,得到多壁碳纳米管-分子印迹传感器。用循环伏安法、交流阻抗法和石英晶体微天平技术对印迹膜进行了表征,膜厚为12.3 nm。K3[Fe(CN)6]的相对峰电流与盐酸克伦特罗的浓度在4.0×10-8～6.6×10-6 mol/L范围内呈线性关系,检测限为8.1×10-9 mol/L。选择性实验表明传感器对结构类似物具有较强的抗干扰能力。此传感器可用于猪肉中盐酸克伦特罗的测定,加标回收率为101.3%～107.9%。     

Quantum dots based electrochemiluminescent immunosensor by coupling enzymatic amplification for ultrasensitive detection of clenbuterol

An ultrasensitive electrochemiluminescence (ECL) immunosensor based on CdSe quantum dots (QDs) has been designed for the detection of clenbuterol. The immunosensor was fabricated by layer by layer and characterized with atomic force microscopic images (AFM) and electrochemical impedance spectra (EIS). In oxygen-saturated pH = 9.0 Tris-HCl buffer, a strong ECL emission of QDs could be observed during the cathodic process due to the H₂O₂ product from electrochemical reduction of dissolved oxygen. Upon the formation of immunocomplex, the second antibody labeled with horseradish peroxidase was simply immobilized on the electrode surface. The ECL emission decreased since steric hindrance of the immunocomplex slowed down the electron-transfer speed of dissolved oxygen, and also could be greatly amplified by an enzymatic cycle to consume the self-produced coreactant. Using clenbuterol as model analyte, the ECL intensity was determined by the concentration of competitive immunoassay of clenbuterol with a wide calibration in the range of 0.05 ng mL⁻¹ to 1000 ng mL⁻¹, and a low detection limit was 0.02 ng mL⁻¹. The immunosensor shows good stability and fabrication reproducibility. It was applied to detecting practical samples with the satisfactory results. This immunosensing strategy opens a new avenue for detection of residue and application of QDs in ECL biosensing.