Application of Novel Zn‐Ferrite Modified Glassy Carbon Paste Electrode as a Sensor for Determination of Cd(II) in Waste Water

This paper describes the preparation of a new sensor based on Zn‐ferrite modified glassy carbon paste electrode and its electrochemical application for the determination of trace Cd(II) ions in waste waters using differential pulse anodic stripping voltammetry (DPASV). Different Zn/Ni ferrite nanoparticles were synthesized and characterized using scanning electron microscopy (SEM) and X‐ray powder diffraction (XRPD). The prepared ferrite nanoparticles were used for the preparation of Zn‐ferrite‐modified glassy carbon paste electrode (ZnMGCPE) for determination of Cd(II) at nanomolar levels in waste water at pH 5. The different parameters such as conditions of preparation, Zn²⁺/Ni²⁺/Fe²⁺ ratio and electrochemical parameters, percentage of modifier, accumulation time, pH and accumulation potential were investigated. Besides, interference measurements were also evaluated under optimized parameters. The best voltammetric response was observed for ZnFe₂O₄ modifier, when the percentage of modifier was 3 %, accumulation time 9 min, pH of supporting electrolyte 5 and accumulation potential ?1.05 V. Thus prepared electrode displays excellent response to Cd(II) with a detection limit of 0.38 ppb, and selective detection toward Cd(II) was achieved.     

MCE‐electrochemical detection for following interactions of ssDNA and dsDNA with methylene blue

The interaction between the organic dye, methylene blue and DNA has been studied by MCE with electrochemical detection. Interaction produces two different signals, one corresponding to free methylene blue and other, for the complex methylene blue–DNA. The hybridization between a ssDNA and a complementary sequence, specific to the severe acute respiratory syndrome virus, has been performed and studied in a thermoplastic olefin polymer of amorphous structure CE‐microchip with an end‐channel gold wire detector. Moreover, studies with a longer dsDNA, an expression vector involved in the transitory or stable expression in mammals cells, pFLAG‐CMV4, has also been performed.     

Interactions of Dissolved dsDNA with Intercalating Drug by Anodic Voltammetry and Spectroscopy. Influence of pH

The interactions of C‐1305 (5‐dimethylaminopropylamino‐8‐hydroxy‐6H‐v‐triazolo[4,5,1‐de]acridin‐6‐one) with DNA were studied using differential pulse voltammetry and UV‐vis spectroscopy. C‐1305 interacts with dsDNA in two ways: by intercalation and by binding to the minor‐groove. For the intercalation at physiological pH (7.4) the values of the binding constant, K₁, and the binding‐site size, n₁, equal 3.36×10⁵ M^?1 and 2.5, respectively. For the weak interactions the K₂ and n₂ parameters equal 0.18×10⁵ M^?1 and 4. In the presence of excess NaCl the weak interactions do not vanish, therefore they are assigned to the minor groove binding. Substantial and complex is the influence of pH.     

Microcystin-(Leucine-Arginine) Immunosensor Based on Iron(II,III) Magnetic Nanoparticles

An electrochemical immunosensor for microcystin-(leucine-arginine) based on magnetic bionanoparticles and iron(II, III) oxide was developed. The bionanoparticles were prepared by cross-linking antibodies of microcystin-(leucine-arginine) and amino-functionalized magnetic iron(II, III) oxide nanoparticles with glutaraldehyde, followed by immobilization on the surface of a magnetic electrode. The immunosensor was based on the model of direct competition, as microcystin-(leucine-arginine) and horseradish peroxidase-conjugated microcystin-(leucine-arginine) competitively combined with immobilizing antibodies. The peak current of differential pulse voltammetry (DPV) decreased with an increase of microcystin-(leucine-arginine) concentration after antigen-antibody reaction. When the background current was stabilized, the anodic peak current response and change in peak response were recorded. Under the optimized conditions, the change in response was proportional to the microcystin-(leucine-arginine) concentration between 0.010 and 100 µg/L with a limit of detection equal to 0.009 µg/L. Amperometry was adopted to determine microcystin-(leucine-arginine); the linear dynamic range was 0.10 to 100 µg/L with a detection limit of 0.08 µg/L. The method was successfully applied in the determination of microcystin-(leucine-arginine) in river water and the recoveries were between 90.2% and 110.5%.     

Microplate electrochemical DNA detection for phosphinothricin acetyltransferase gene sequence with cadmium sulfide nanoparticles

An electrochemical DNA detection method for the phosphinothricin acetyltransferase (PAT) gene sequence from the transgenetic plants was established by using a microplate hybridization assay with cadmium sulfide (CdS) nanoparticles as oligonucleotides label. The experiment included the following procedures. Firstly target PAT ssDNA sequences were immobilized on the polystyrene microplate by physical adsorption. Then CdS nanoparticle labeled oligonucleotide probes were added into the microplate and the hybridization reaction with target ssDNA sequences took place in the microplate. After washing the microplate for three times, certain amounts of HNO₃ were added into the microplate to dissolve the CdS nanoparticles anchored on the hybrids and a solution containing Cd²⁺ ion was obtained. At last differential pulse anodic stripping voltammetry (DPASV) was used for the sensitive detection of released Cd²⁺ ion. Based on this principle a sensitive electrochemical method for the PAT gene sequences detection was established. The voltammetric currents of Cd²⁺ were in linear range with the target ssDNA concentration from 5.0 × 10^− 13 to 1.0 × 10^− 10 mol/L and the detection limit was estimated to be 8.9 × 10^− 14 mol/L (3σ). The proposed method showed a good promise for the sensitive detection of specific gene sequences with good selectivity for the discrimination of the mismatched sequences.     

Study of redox behavior of Cd(II) and interaction of Cd(II) with proline in the aqueous medium using cyclic voltammetry

The redox behavior of Cd(II) and the interaction of Cd(II) with cyclic amino acid, proline, have been studied in 0.1 M KCl, 0.1 M NaClO₄ and acetate buffer of different pH. The CVs were recorded at glassy carbon electrode within the potential window 200 and ?1500 mV. The reference and counter electrode used were Ag/AgCl and Pt wire, respectively. The cyclic voltammograms show one pair of cathodic and anodic peaks for the Cd(II)/Cd(0) system indicating the involvement of two electron transfer processes. The peak potential shift and charge transfer rate constant (k_f) values strongly support the interaction between metal and ligand. The higher value of peak current ratio and peak potential separation (ΔE) indicate that the systems are quasireversible. The effect of supporting electrolyte and concentration of electro active species on the interaction were also studied.     

Development of a New Label‐free,Indicator‐free Strategy toward Ultrasensitive Electrochemical DNA Biosensing Based on Fe3O4 Nanoparticles/Reduced Graphene Oxide Composite

Electrochemistry offers sensitivity, selectivity and low cost for fabrication of sensors capable of detection of selected DNA targets or mutated genes associated with human disease. In this work, we have developed a novel label‐free, indicator‐free strategy of electrochemical DNA sensor based on Fe₃O₄ nanoparticles/reduced graphene oxide (Fe₃O₄/r‐GO) nanocomposite modified electrode. By using Fe₃O₄/r‐GO nanocomposite as a substrate to immobilize probe DNA and subsequent hybridization with target sequence to form dsDNA, a great signal amplification was achieved through measuring changes in DPV peak current of underlying Fe(II)/Fe(III) redox system. With the remarkable attomolar sensitivity and high specificity and at the same time, great simplicity, the proposed strategy may find great applications in different DNA assay fields.     

Voltammetric and Impedimetric Detection of Interaction Between Dacarbazine and Nucleic Acids

Dacarbazine (DTIC) is a chemotherapy drug that is used for the treatment of Hodgkin's lymphoma, malignant melanoma, childhood solid tumors and soft tissue sarcoma. The surface confined interaction between DTIC and nucleic acids was investigated for the first time in this study by using both differential pulse voltammetry (DPV) and electrochemical impedance spectroscopy (EIS) in combination with disposable pencil graphite electrodes. The oxidation signals of DTIC and guanine were measured before and after interaction process using DPV technique. The interaction of DTIC with nucleic acids; poly[A], poly[G], or double stranded of poly[A]‐poly[T] and poly[G]‐poly[C] was also examined using DPV. Furthermore, EIS technique was utilized for detection of the interaction between DTIC and nucleic acids; ssDNA/dsDNA, poly[A], poly[G], or double stranded poly[A]‐poly[T] and poly[G]‐poly[C].     

Simultaneous determination of lead(II) and cadmium(II) at a diacetyldioxime modified carbon paste electrode by differential pulse stripping voltammetry

A simple and effective chemically modified carbon paste electrode (CMCPE) for the simultaneous determination of lead(II) and cadmium(II) was developed in this work. The electrode was prepared by the addition of diacetyldioxime into a carbon paste mixture. Pb²⁺ and Cd²⁺ were preconcentrated on the surface of the modified electrode by complexing with diacetyldioxime and reduced at a negative potential (−1.10 V). Then the reduced products were oxidized by differential pulse stripping. The fact that two stripping peaks appeared on the voltammograms at the potentials of −0.65 V (Cd²⁺) and −0.91 V (Pb²⁺) demonstrates the possibility of simultaneous determination of Pb²⁺ and Cd²⁺. Under the optimized working conditions, calibration graphs were linear in the concentration ranges of 1.0×10⁻⁷-1.5×10⁻⁵ mol l⁻¹ (Pb²⁺) and 2.5×10⁻⁷-2.5×10⁻⁵ mol l⁻¹ (Cd²⁺), respectively. For 5 min preconcentration, detection limits of 1×10⁻⁸ mol l⁻¹ (Pb²⁺) and 4×10⁻⁸ mol l⁻¹ (Cd²⁺) were obtained at the signal noise ratio (SNR) of 3. To evaluate the reproducibility of the newly developed electrode, the measurements of 5×10⁻⁷ mol l⁻¹ Pb²⁺ and Cd²⁺ were parallel carried out for six times at different electrodes and the relative standard deviations were 2.9% (Pb²⁺) and 3.2% (Cd²⁺), respectively. Interferences by some metals were investigated. Only Ni²⁺ and Hg²⁺ apparently affected the peak currents of Pb²⁺ and Cd²⁺. The diacetyldioxime modified carbon paste electrode was applied to the determination of Pb²⁺ and Cd²⁺ in water samples. The results indicate that this electrode is sensitive and effective for the simultaneous determination of Pb²⁺ and Cd²⁺.     

Lable‐Free Electrochemical DNA Sensor Based on Gold Nanoparticles/Poly(neutral red) Modified Electrode

We present a new strategy for the label‐free electrochemical detection of DNA hybridization based on gold nanoparticles (AuNPs)/poly(neutral red) (PNR) modified electrode. Probe oligonucledotides with thiol groups at the 5‐end were covalently linked onto the surface of AuNPs/PNR modified electrode via S‐Au binding. The hybridization event was monitored by using differential pulse voltammetry (DPV) upon hybridization generates electrochemical changes at the PNR‐solution interface. A significant decrease in the peak current was observed upon hybridization of probe with complementary target ssDNA, whereas no obvious change was observed with noncomplementary target ssDNA. And the DNA sensor also showed a high selectivity for detecting one‐mismatched and three‐mismatched target ssDNA and a high sensitivity for detecting complementary target ssDNA, the detection limit is 4.2×10^?12 M for complementary target ssDNA. In addition, the DNA biosensor showed an excellent reproducibility and stability under the DNA‐hybridization conditions.     

Hg(II) immobilized MWCNT graphite electrode for the anodic stripping voltammetric determination of lead and cadmium

The preparation of Hg(II)-modified multi walled carbon nanotube (MWCNT) by reaction of oxidized MWCNT with aqueous HgCl₂ was carried out. The Hg(II)-modified multi walled carbon nanotube (Hg(II)/MWCNT) dispersed in Nafion solution was used to coat the polished graphite electrode surface. The Hg(II)/MWCNT modified graphite electrode was held at a cathodic potential (−1.0 V) to reduce the coordinated Hg(II) to Hg forming nanodroplets of Hg. The modified electrode was characterized by FESEM/EDAX which provided useful insights on the morphology of the electrode. The SEM images showed droplets of Hg in the size of around 260 nm uniformly distributed on the MWCNT. Differential pulse anodic stripping voltammetry (DPASV) and electrochemical impedance spectroscopy were used to study the Hg(II) binding with MWCNT. Differential pulse anodic stripping voltammetry of ppb levels of cadmium and lead using the modified electrode yielded well-defined peaks with low background current under a short deposition time. Detection limit of 0.94 and 1.8 ng L⁻¹ were obtained following a 3 min deposition for Pb(II) and Cd(II), respectively. Various experimental parameters were characterized and optimized. High reproducibility was observed from the RSD values for 20 repetitive measurements of Pb(II) and Cd(II) (1.7 and 1.9%, respectively). The determination of Pb(II) and Cd(II) in tap water and Pb(II) in human hair samples was carried out. The above method of fabrication of Hg(II)/MWCNT modified graphite electrode clearly suggests a safe route for preparing Hg immobilized electrode for stripping analysis.     

Pencil Lead Electrode Modified with Hemoglobin Film as a Novel Biosensor for Nitrite Determination

In the present paper, the electrochemical reduction of nitrite at a hemoglobin modified pencil lead electrode (Hb/PLE) is described. The electrochemical properties of nitrite were studied by cyclic voltammetry and chronoamperometry. Results showed that the hemoglobin film has an excellent electrochemical activity towards the reduction of nitrite. By using voltammetric and chronoamperometric methods, α, n_α and n were calculated. Then the ability of the electrode for nitrite determination was investigated using differential pulse voltammetry. The electrocatalytic reduction peak currents were found to be linear with the nitrite concentration in the range from 10 to 220 µM with a detection limit of 5 µM. The relative standard deviation is 2 % for 3 successive determinations of a 100 µM nitrite solution. This modified electrode was successfully used for the detection of low amounts of NO₂^? in spinach sample and a spiked sample of tap water.     

Simultaneous determination of chromium(III) and cadmium(II) by differential pulse anodic stripping voltammetry on a stannum film electrode

A stannum film electrode has been developed for the simultaneous determination of trace levels of chromium(III) and cadmium(II) by differential pulse anodic stripping voltammetry (DPASV). The stannum film electrode was generated in situ by depositing simultaneously the stannum film and the metals obtained by reduction of Cd(II) and Cr(III) at −1.4 V on a glassy carbon electrode. Then, the reduced products were oxidized by scanning the potential of the electrode from −1.4 to −0.4 V using DPASV. The electrode exhibited well-defined and separated stripping signals for both metals accompanied with a low background contribution. The possible mechanism of this design was proposed. Under the optimized working conditions, the detection limit was 2.0 and 1.1 μg l⁻¹ for Cr(III) and Cd(II) at a deposition time of 3 min. Finally, the stannum film electrode was successfully applied to the determination of Cd(II) in tap water with satisfactory results.     

Electrochemical Recognition of Chiral Molecules with Poly(4‐bromoaniline) Modified Gold Electrode

A poly(4‐bromoaniline) (PBA) film is electrochemically synthesized on a gold electrode for the recognition of amino acids enantiomers. Scanning electron microscopy measurements show that the porous PBA films are made up of nano‐ribbons. At the PBA modified Au electrode differential pulse voltammograms of L ‐ and D ‐glutamic acids not only have very different current densities, but also produce different waveforms, providing an intuitive way to differentiate the two chiral molecules. Similar results are obtained in analyzing L ‐ and D ‐aspartic acids. Control experiments suggest that the observed sensing behavior arises from synergistic interactions between Au and the PBA film, where polymerization at the meta‐position creates a steric structure needed for differentiating chiral molecules.     

Simultaneous electrochemical DNA hybridization assay for PAT and FMV 35S gene sequence using quantum dots as labels

An electrochemical method for the simultaneous detection of two different DNA sequences from PAT and FMV 35S gene sequence using CdS and PbS quantum dots （QDs） as labels was described. The QDs were readily functionalized with oligonucleotides as electrochemical DNA probes and selectively hybridized to the complementary sequences immobilized on the microplate. The QDs anchored on the hybrids were dissolved in the solution by the oxidation of HNO3 and further detected by a sensitive differential pulse anodic stripping voltammetric method （DPASV）. The DPASV signals of the oxidation of Cd^2＋ and Pb^2＋ ions present in the solution were different and reflected the identity of corresponding ssDNA targets sequences.     

Application of Cupferron‐lead(II) Complex for the Electrochemical Determination of dsDNA

Based on the interaction of cupferron and lead(II) complex [Cup‐Pb(II)] with double‐stranded DNA (dsDNA) a new voltammetric method for the detection of DNA was described in this paper. In pH 4.0 HAc‐hexamine buffer solution, [Cup‐Pb(II)] complex showed a sensitive second order derivative polarographic reductive peak at ‐0.554 V (vs. SCE). After the addition of dsDNA into [Cup‐Pb(II)] mixture solution the reductive peak current decreased with the positive shift of reductive peak potential, which was the typical characteristic of intercalation mode. Under the optimum conditions, the decrease of reductive peak current was directly proportional to the dsDNA concentration in the range from 1.0 to 25.0 mg/L with the linear regression equation as ΔIp″ (nA) = 129.30 + 62.51 C (mg/L) (n = 13, γ = 0.991). The detection limit of 0.90 mg/L (3σ) and the relative standard derivation (RSD) of 2.43% for 10 parallel determinations of 10.0 mg/L dsDNA were found. The method was successfully applied to synthetic samples with good results, and the stoichiometry of dsDNA with [Cup‐Pb(II)] complex was calculated by the voltammetic data with the binding number as 2 and the binding constant as 2.82 × 10⁹.     

Pulsed amperometric detection of DNA with an ssDNA/polypyrrole-modified electrode

Pulsed amperometric detection (PAD) of target DNA with platinum electrodes modified by single-stranded DNA (ssDNA) entrapped within polypyrrole (ssDNA/Ppy) is reported for the first time. Single-stranded DNA 20-mers complementary to the target DNA were used to construct the DNA biosensors. Polymerase chain reaction (PCR) amplified bovine leukaemia virus (BLV) provirus DNA was used as target DNA. Electrochemical impedance spectroscopic (EIS) investigation of ssDNA/Ppy before and after incubation in target DNA-containing sample revealed significant changes in terms of an imaginary (Z) vs. a real (Z) component. The PAD results were in good agreement with EIS investigations. The PAD method was selected, because it does not require such sophisticated equipment as it is used to perform EIS and the results obtained can be more easily estimated. Optimum conditions for performing PAD and evaluating an analytical signal were elaborated. No label-binding step was necessary for detection of target DNA in PCR-amplified amplicons and detection time was reduced by as much as 30–35 min. The changes of PAD signals were at least 6–7 times higher if ssDNA/Ppy-modified electrodes instead of blank Ppy-modified electrodes were incubated in the target DNA solutions. If ssDNA/Ppy modified electrodes were incubated in non-complementary (control) DNA solution changes in PAD signals were smaller than those detected after incubation in complementary (target) DNA-containing solution by a factor of at least 6–8.     

用于肿瘤标志物现场快速检测的便携式仪表的研制

针对肿瘤标志物高灵敏度现场快速检测的需求,将电化学检测技术与电子技术相结合,采用差分脉冲伏安法(Differential pulse voltammetry,DPV)研制了一种可用于肿瘤标志物现场快速检测的便携式仪表,检测电压和电流的分辨率分别为0.8 mV和1nA.结合实验室自制微流控纸芯片,利用该便携式仪表对肿瘤标志物癌胚抗原(Carcinoembryonic antigen,CEA)进行检测,实验结果表明,在1～500 μg/L浓度范围内,DPV峰值电流响应与CEA抗原浓度对数呈线性关系,线性相关系数为0.998,检出限为10 pg/mL.根据抗原抗体特异性结合和电化学检测原理,检测到电化学反应的微弱电流后,仪表可以根据已经标定的电流与浓度之间的比例关系自动计算出肿瘤标志物的浓度.此便携式仪表具有检测灵敏度高、检出限低等优点,可广泛应用于肿瘤标志物的即时检测.     

Voltammetric Determination of Hemoglobin Using a Pencil Lead Electrode

In this paper the electrochemical behavior of hemoglobin (Hb) immobilized on a pencil lead electrode (PLE) was investigated. Immobilization of Hb on the pencil lead electrode was performed by nonelectrochemical and electrochemical methods. In phosphate buffer solution with pH 7.0 Hb showed a pair of well‐defined and nearly reversible redox waves (the anodic and cathodic peak potentials are located at ?0.18 V and ?0.22 V, respectively). The dependence of the anodic peak potential (E_pa) on the pH of the buffer solution indicated that the conversion of Hb? Fe(III)/Hb? Fe(II) is a one‐electron‐transfer reaction process coupled with one‐proton‐transfer. In addition the effect of scan rate on peak currents and peak separation potential was investigated and electrochemical parameters such as α and k_s were calculated. In the second part of this work, the ability of the electrode for determination of Hb concentration was investigated. The results showed a linear dynamic range from 0.15 to 2 µM and a detection limit of 0.11 µM. The relative standard deviation is 4.1 % for 4 successive determinations of a 1 µM Hb solution.     

基于铜离子与DNA相互作用的铜离子检测

利用铜离子(Cu~(2+))可与DNA分子中的碱基相互作用形成络合物的性质,将Cu~(2+)富集在DNA修饰电极表面,进而采用微分脉冲伏安法(DPV)实现了铜离子的检测.此外,由于乙二胺四乙酸(EDTA)对Cu~(2+)具有更强的络合能力,富集于DNA修饰电极表面的Cu~(2+)很容易被洗脱液中的EDTA络合,从而实现修饰电极的再生和重复利用.实验结果表明,在最佳实验条件下,Cu~(2+)浓度在2.0×10-6~1.0×10-5mol/L和2.0×10-5~1.0×10-4mol/L范围内与其相对还原峰电流强度(I-I0)呈良好的线性关系,且该传感器简单、稳定,可循环使用.