纳米金颗粒增强信号的电化学生物传感器用于谷胱甘肽和半胱氨酸的检测

构建了一种高灵敏检测谷胱甘肽(GSH)和半胱氨酸(Cys)的新型电化学生物传感器. 先将富含T碱基的DNA1和DNA2探针分别修饰在金电极和纳米金颗粒(AuNPs)上, 再加入Hg²⁺, 通过形成T-Hg²⁺-T结构使AuNPs结合到金电极表面. 当加入GSH(或Cys)后, GSH(或Cys)可以竞争结合T-Hg²⁺-T结构中的Hg²⁺, 使AuNPs离开电极表面. 由于AuNPs上修饰的DNA探针能够静电吸附大量电活性物质六氨合钌(RuHex), 因此该过程可引起计时电量信号的显著变化, 据此实现了GSH(或Cys)的高灵敏检测. 该传感器的检出限达10 pmol/L, 比荧光法或比色法降低了2~3个数量级. 实验结果表明, 该传感器具有较好的选择性.     

Determination of Imidacloprid Based on the Development of a Glassy Carbon Electrode Modified with Reduced Graphene Oxide and Manganese (II) Phthalocyanine

An electrochemical sensor of glassy carbon electrode modified with reduced graphene oxide and manganese (II) phthalocyanine (GCE/rGO/MnPc) was developed as an effective alternative in the determination of imidacloprid in honey samples. The peak current variation obtained with the proposed sensor, in the presence of imidacloprid, was higher compared to the bare GCE. The followed experimental conditions were optimized: reduced graphene oxide concentration (2.0 mg mL^?1), manganese (II) phthalocyanine concentration (1.5 mg mL^?1), electrolyte pH (6.5) and electrolyte concentration (1,50 mol L^?1). The study also showed that the process of reduction of imidacloprid is irreversible and diffusion‐controlled, with a single reduction peak of approximately ?0.9 V corresponding to the reduction of the nitro group (?NO2) present in the structure, generating a derived from hydroxylamine, in a process involving about four electrons. The determination of imidacloprid in honey samples exhibited recovery values within the EPA range (between 90.5 and 101.9 %). The proposed sensor GCE/rGO/MnPc can be used as an effective alternative in the determination of imidacloprid in honey samples.     

Design of a Sensitive Electrochemical Sensor Based on Ferrocene-reduced Graphene Oxide/Mn-spinel for Hydrazine Detection

Herein, we report construction of a ferrocene-reduced graphene oxide-Mn spinel modified glassy carbon electrode (Fc−G/Mn₃O₄/GCE) as a sensitive electrochemical probe for hydrazine detection via its oxidation. The synergistic effect of ferrocene, graphene oxide and Mn₃O₄ provides it a great electrocatalytic effect. The electrochemical investigations of Fc−G/Mn₃O₄/GCE were studied using cyclic voltammetry, while differential pulse voltammetry was utilized for recording the electrocatalytic sensing of hydrazine. The prepared Fc−G/Mn₃O₄ offers a platform for sensitive and selective detection of low-level hydrazine in two linear ranges from 0.045 to 108 μM and 108 to 653 μM with limit of detection 8.5 nM. Real sample analysis was also performed in local industrial water samples with satisfactory recovery results.     

Electrochemical Probe of the Reduced Graphene Oxide Modified by Bare Gold Nanoparticles Functionalized Zr(IV)-based Metal-organic Framework for Detecting Nitrite

Widely presented nitrite in drinking water, food and even physiological system endangers human health. Here,bare gold nanoparticles functionalized Zr-based metal-organic framework modified reduced graphene oxide (GNPs/UiO-66-NH₂/rGO) nanocomposites were prepared by hydrothermal method. This experiment studies the morphology, composition, structure and electrochemical behavior of the sensor. The experimental results show that the sensor has a peak potential of 0.9 V, the concentration range of NO₂⁻ is 5.0 μM to 768 μM, the linear regression equation of the calibration curve is I_pa=0.3646+0.00642 C (R²=0.9998), and the LOD is as low as 3.7 μM (S/N=3). Therefore, an electrochemical sensor platform for trace detection of NO₂⁻ was successfully constructed.     

Electropolymerized Manganese Tetraaminophthalocyanine Thin Films onto Platinum Ultramicroelectrode for the Electrochemical Detection of Peroxynitrite in Solution

Peroxynitrite, ONOO^? also so‐called PON, is a very powerful oxidant and cytotoxic agent produced in biological systems by the recombination of nitric oxide and superoxide anion radical. Most of the techniques for assaying PON (chemiluminescence, fluorescence, UV‐visible spectroscopy, immunochemistry and EPR ) use indirect methods relying on measurements of secondary species. We report in this study the calibration of a chemically modified Pt ultramicroelectrode by electropolymerized manganese tetraaminophthalocyanine film (MnTAPc) for the determination of PON in aqueous solution. The obtained result allows showing for the first time a real‐time calibration curve of the amperometric determination of stable PON in aqueous solution. The sensitivity of the sensor is 14.6 nA mM^?1 and its detection limit is 5 μM.     

A Sensitive Nanoporous Gold-Based Electrochemical DNA Biosensor for Escherichia coli Detection

A sensitive electrochemical DNA biosensor based on a mixed monolayer structure self-assembled at nanoporous gold (NPG) electrode surface was prepared for Escherichia coli (E. coli) detection. The NPG was fabricated on gold electrode, onto which thiolated oligonucleotides (SH-DNA) and mercaptohexanol (MCH) were covalently linked forming a mixed self-assembled monolayer (SAM). The hybridization between the SH-DNA/MCH modified biosensor and E. coli DNA was monitored with differential pulse voltammetry measurement using methylene blue (MB) as the hybridization indicator. The biosensor can detect 1 × 10^?12 M DNA target and 50 cfu/μL E. coli without any nucleic acid amplification steps. The detection limit was lowered to 50 cfu/mL after 5.0 h of incubation.     

A Sensitive Electrochemical Biosensor for Detection of Histone Deacetylase Activity Using an Acetylated Peptide

A sensitive electrochemical biosensor was developed for activity detection of histone deacetylase sirtuin2 (SIRT2) using an acetylated peptide substrate. This substrate could be recognized by anti‐acetylated peptide antibody, which could be detected using secondary antibody conjugated alkaline phosphatase which provided an amplified electrochemical signal. In the presence of SIRT2, the substrate was deacetylated, resulting in a decreased electrochemical signal that was correlated to the concentration of SIRT2. Under optimized conditions, the biosensor exhibited a wide linear range from 1 nM to 500 nM with a detection limit of 0.1 nM. The proposed biosensor was also used for detection of SIRT2 inhibitor.     

Electrochemical Biosensors for Cancer Biomarkers Detection: Recent Advances and Challenges

Biomarkers are described as characteristics that provide information about biological conditions whether normal or pathological. Detection of biomarkers at the earliest stage of the cancer is of utmost importance for clinical diagnosis. Electrochemical biosensors allow detecting the low levels of specific analytes in blood, urine or saliva and providing a sensitive approach for direct measurement for cancer biomarker detection. Moreover, the integration of electrochemical devices with nanomaterials, such as carbon nanotubes, gold and magnetic particles offer amplification and multiplexing capabilities for simultaneous measurements of cancer biomarkers very sensitively. This review summarizes the recent developments of electrochemical biosensors systems for the detection of cancer biomarkers with emphasis on voltammetric, amperometric and impedimetric biosensors. A special attention is paid to aptamers and miRNAs that are very promising for the ultra‐sensitive and specific cancer biomarker detection.     

Simple Analysis of Glutathione in Human Colon Carcinoma Cells and Epidermoid Human Larynx Carcinoma Cells by HPLC with Electrochemical Detection

Here, we provide an extremely simple, rapid, direct, sensitive and specific method to quantify, for the first time in human colon carcinoma cells (HT29) and epidermoid human larynx carcinoma cells (HEp-2), the intracellular glutathione (GSH) using an electrochemical detector coupled to a high performance liquid chromatograph (HPLC-ECD). GSH determination in cancer cells are of valuable interest because GSH has been implicated in the development of resistance to several anticancer drugs. Separation of GSH was performed on a Alltima C18 column using a binary pre-mixed mobile phase of methanol-NaH₂PO₄ (10 mM, pH 3.0 with phosphoric acid) (2:98, v/v). GSH was detected with an oxidation potential of +500 mV. The limit of detections was 0.30 pMol and good linearity (r = 0.9988) was found. The intra-day and the inter-day recoveries were 97.1–101.3% and 98.2–101.8% respectively, whereas the accuracies were less than 2.56% and 3.02% respectively. The usefulness of the method was established by subjecting HT29 and HEp-2 cells to an oxidant stress generated by menadione, a substance able to decrease GSH level in cells. The experiments show that the HPLC-ECD method developed could represent an useful alternative to the existing procedures since its simplicity and rapidity.     

An Electrochemical Sensor Based on Electropolymerization of ß‐Cyclodextrin and Reduced Graphene Oxide on a Glassy Carbon Electrode for Determination of Neonicotinoids

An electrochemical sensor of glassy carbon electrode modified with reduced graphene oxide and β‐cyclodextrin (GCE/rGO/β‐CD) was developed as an effective alternative in the determination of neonicotinoid insecticides, imidacloprid, clothianidin and thiamethoxam, in honey samples. The peak current variation obtained with the proposed sensor was higher compared to the bare GCE in all the analytes. In the determination of imidacloprid the response increased by 1300 %, clothianidin by 670 % and thiametoxam by 630 %. In addition, the optimization of the experimental conditions provided the construction of a sensor with greater sensitivity. The study of interferers showed that inorganic ions (Ca²⁺, Mg²⁺, Fe²⁺, K⁺, Na⁺, e NH₄⁺) and other insecticides (acetamiprid and dinotefuran) did not influence the reduction of imidacloprid, clothianidin and thiamethoxam. The determination of imidacloprid, clothianidin and thiamethoxam in honey samples exhibited recovery values within the EPA range (between 107.75 and 116 %). In conclusion, the developed sensor GCE/rGO/β‐CD proved to be an effective alternative in the determination of neonicotinoid insecticides in honey samples.     

Total Determination of Estrogenic Phenolic Compounds in River Water Using a Sensor Based on Reduced Graphene Oxide and Molecularly Imprinted Polymer

The contamination of water and wastewater by emerging pollutants, due to the anthropogenic activities, are an environmental problem that generates several negative impacts. In this range of species, steroids have gaining notoriety because their action of endocrine‐disruption. In this work, they are called estrogenic phenolic compounds (EPCs): estrone (E₁), estradiol (E₂), ethinyl estradiol (EE₂) and estriol (E₃), for determination using an electrochemical sensor based on reduced graphene oxide (rGO) and molecularly imprinted polymer (MIP). The analytical method developed, allied with the experimental and operational optimizations, proved to be effective for the total quantification of the EPCs in river water. The method shows sensitivity of 1.12 μA/μmol L⁻¹, detection limit of 26.8 nmol L⁻¹ and linear range of 0.16–15 μmol L⁻¹. The similar electrochemical behavior of the four compounds studied (E₁, E₂, EE₂ and E₃) and the efficiency of the modified composite (rGO, MIP) in the fabrication of the sensor resulted in high electrical conductivity and selective adsorptivity, respectively.     

用于DNA杂交检测的丝网印刷型生物传感器的研究

将单链DNA(ssDNA)固定到丝网印刷碳电极上构成电化学DNA传感器,采用电化学指示剂,建立DNA杂交的检测方法.Co(phen)33+电化学指示剂通过钴盐与配体邻菲罗啉络合制备,采用等离子发射光谱法(ICP-AES)和核磁共振法(NMR)表征功能基团,采用循环伏安法(CV)分析指示剂的电化学特性,并以此为基础研究ssDNA在电极表面的固定及DNA杂交过程.本研究探讨了直接吸附、静电吸附与键合等3种ssD-NA在电极表面的固定方法,结果表明,静电吸附法和键合法具有较高的ssDNA固定量,采用静电吸附法固定探针的电极杂交目标DNA后,Co(phen)33+易于嵌入双链DNA (dsDNA)中,CV峰电流(ip)信号随目标DNA浓度增加.本研究采用静电吸附ssDNA的电极检测DNA杂交,实验表明,当探针固定液中ssDNA浓度为5 mg/L时,目标DNA浓度在6.65×10- 8～4.26× 10-6mol/L范围内,Co(phen)33+在dsDNA修饰电极上ip值与DNA浓度呈良好的线性关系,R2为0.9819.本研究为建立新的微生物分子分型手段提供了初步依据.     

Dual Signal Amplification Electrochemical Biosensor for Lead Cation

Herein, a sensitive electrochemical Pb²⁺ sensor was developed which based on DNA‐functionalized Au nanoparticles(AuNPs) and nanocomposite modified electrode. The DNA‐functionalized AuNPs includes two types of DNA, namely a Pb²⁺‐mediated DNAzyme comprising a biotin labeled‐enzyme DNA and a substrate strand DNA with a typical stem‐loop structure, and a ferrocene‐labeled linear signal DNA. Without Pb²⁺, the hairpin loop impeded biotin binding to avidin on the electrode. However,when the goal Pb²⁺ exists, the substratum strand was divided into two fragments that lead to the enzyme strand was substratumed on the electrode and biotin was admited by avidin, bringing about DNA‐functionalized AuNP(AuNPs) deposition on the electrode surface.The differential pulse voltammetry (DPV) was used to measure electrochemical response signals connect to signal DNA.For the amplification characters of the DNA‐functionalized AuNPs and nanocomposite, the electrochemical detection signal of Pb²⁺ was greatly improved and revealed high specificity. Under optimum conditions, the resultant biosensor bringed out a high sensitivity and selectivity for the determination of Pb²⁺. The proposed method was able to detect as low as picomolar Pb²⁺ concentrations.     

基于层状双金属氢氧化物的电化学生物传感器研究进展

层状双金属氢氧化物（LDHs）具有开放的二维平面结构和良好的生物相容性,是非常适合于将生物酶固定在电极表面用于生物传感器的主体材料。本文介绍了酶在LDHs材料上的固定方法,综述了近年来基于这类二维层状材料的各种电化学生物传感器的研究进展,讨论了不同类型生物传感器的设计原理和电子传递机理,并对LDHs在电化学生物传感领域...     

Development of an Amperometric Microbial Biosensor Based on Thiobacillus thioparus Cells for Sulfide and Its Application to Detection of Sulfate‐Reducing Bacteria

This paper describes a novel electrochemical microbial biosensor based on Thiobacillus thioparus cells for sulfide detection. The morphology and electrochemical properties of the proposed biosensor were characterized by SEM and cyclic voltammetry, respectively. Working conditions of the microbial biosensor were optimized to obtain good electrochemical performances. Under the optimum conditions, analytical performances were evaluated, and the results suggested that the microbial biosensor could be used for selective detection of sulfide. The microbial biosensor was then successfully applied in detection of sulfate‐reducing bacteria by oxidizing its characteristic metabolite, sulfide, which was accumulated in culture media during bacterial growth.     

Development of a Temperature-pulse Enhanced Electrochemical Glucose Biosensor and Characterization of its Stability via Scanning Electrochemical Microscopy

Glucose oxidase (GOx) is an enzyme frequently used in glucose biosensors. As increased temperatures can enhance the performance of electrochemical sensors, we investigated the impact of temperature pulses on GOx that was drop-coated on flattened Pt microwires. The wires were heated by an alternating current. The sensitivity towards glucose and the temperature stability of GOx was investigated by amperometry. An up to 22-fold increase of sensitivity was observed. Spatially resolved enzyme activity changes were investigated via scanning electrochemical microscopy. The application of short (<100 ms) heat pulses was associated with less thermal inactivation of the immobilized GOx than long-term heating.     

Reduced Graphene Sheets Modified Electrodes for Electrochemical Detection of Sulfide

This paper describes a new electrochemical sensor based on reduced graphene sheets (RGSs) modified glassy carbon electrodes for rapid detection of sulfide. The morphology and electrochemical properties of the RGSs are characterized by atomic force microscopy and cyclic voltammetry. The effects of the scan rates and pH are investigated to evaluate the oxidation processes. Analytical performances of RGSs modified electrodes for direct determination of sulfide in phosphate buffer solutions (PBSs) are also assessed. The RGSs are shown to be viable potential material for sulfide detection as shown by their electrochemical performance.     

Electrochemical DNA Biosensor Based on Graphene and TiO2 Nanorods Composite Film for the Detection of Transgenic Soybean Gene Sequence of MON89788

Based on graphene (GR), TiO₂ nanorods, and chitosan (CTS) nanocomposite modified carbon ionic liquid electrode (CILE) as substrate electrode, a new electrochemical DNA biosensor was effectively fabricated for the detection of the transgenic soybean sequence of MON89788. By using methylene blue (MB) as hybridization indicator for monitoring the hybridization with different ssDNA sequences, the differential pulse voltammetric response of MB on DNA modified electrodes were recorded and compared. Due to the synergistic effects of TiO₂ nanorods and GR on the electrode surface, the electrochemical responses of MB were greatly increased. Under optimal conditions the differential pulse voltammetric response of the target ssDNA sequence could be detected in the range from 1.0×10^?12 to 1.0×10^?6 mol/L with a detection limit of 7.21×10^?13 mol/L (3σ). This electrochemical DNA biosensor was further applied to the polymerase chain reaction (PCR) product of transgenic soybeans with satisfactory results.     

Electrochemical Aptasensors for Biological and Chemical Analyte Detection

Aptamers are short length, single-stranded DNA or RNA affinity molecules which interact with any desired targets such as biomarkers, cells, biological molecules, drugs or chemicals with high sensitivity. They have been extensively employed for medical applications due to having more advantages than the antibodies such as easier preparation and modification, higher stability, lower batch-to-batch variability and cost. Moreover, aptamers can be easily integrated efficiently with sensors, biosensors, actuators and other devices. In this review article, different applications of aptamers for biological and chemical molecules detection within the scope of electrochemical methods were presented with recent studies. In addition, the present status and future perspectives for highly-effective aptasensors for specific and selective analyte detection were discussed. As in stated throughout the review, combining of extraordinary properties of aptamers with the electrochemical-based biosensors could have improved the sensitivity of the assay and reduced limit of detection.     

Electrochemical Sensors for Nitric Oxide Detection in Biological Applications

Nitric oxide (NO) plays an important role in physiological processes and it has been confirmed some human diseases are related to its biological function. Electrochemical sensors provide an efficient way to explore the NO function in biological processes. This review details different kinds of electrochemical sensors used for NO concentration detection between 2008 and 2013 together with their application in biological samples. Four commonly used electrodes and different assisted analysis membranes used for contributions towards the development of the novel sensors were summarized. Electrochemical sensors employed to measure NO concentration in a single cell, cell culture, tissue homogenate, organ, in vivo, human being, as well as in plant were also detailed. The trends of developing novel NO sensors were outlooked in the last part.