Fe3O4 magnetic nanoparticles as peroxidase mimetics and their applications in H2O2 and glucose detection

Artificial enzyme mimetics are a current research interest because natural enzymes bear some serious disadvantages, such as their catalytic activity can be easily inhibited and they can be digested by proteases. A very recently study reported by Yan et al. has proven that Fe(3)O(4) magnetic nanoparticles (MNPs) exhibit an intrinsic enzyme mimetic activity similar to that found in natural peroxidases, though MNPs are usually thought to be biological and chemical inert (Gao, L. Z.; Zhuang, J.; Nie, L.; Zhang, J. B.; Zhang, Y.; Gu, N.; Wang, T. H.; Feng, J.; Yang, D. L.; Perrett, S.; Yan, X. Y. Nat. Nanotechnol. 2007, 2, 577-583). In the present work, we just make use of the novel properties of Fe(3)O(4) MNPs as peroxidase mimetics reported by Yan et al. to detect H(2)O(2). The Fe(3)O(4) MNPs were prepared via a coprecipitation method. The as-prepared Fe(3)O(4) MNPs were then used to catalyze the oxidation of a peroxidase substrate 2,2'-azino-bis(3-ethylbenzo-thiazoline-6-sulfonic acid) diammonium salt (ABTS) by H(2)O(2) to the oxidized colored product (see eq 1) which provides a colorimetric detection of H(2)O(2). As low as 3 x 10(-6) mol/L H(2)O(2) could be detected with a linear range from 5 x 10(-6) to 1 x 10(-4) mol/L via our method. More importantly, a sensitive and selective method for glucose detection was developed using glucose oxidase (GOx) and the as-prepared Fe(3)O(4) MNPs. The detection platforms for H(2)O(2) and glucose developed in the present work not only further confirmed that the Fe(3)O(4) MNPs possess intrinsic peroxidase-like activity but also showed great potential applications in varieties of simple, robust, and easy-to-make analytical approaches in the future.     

Preparation, characterization, and application of an enzyme-immobilized magnetic microreactor for flow injection analysis

Enzyme-immobilized magnetic microparticles (EMMP) have been prepared for use as a microreactor in flow injection analysis (FI). The microparticles were directly injected into the FI system. Their retention occurred within the flow line by small permanent magnets located near the detector. The analytical utility of this concept was illustrated by the assay of glucose using glucose oxidase (GOx), immobilized microparticles, and amperometric detection of liberated hydrogen peroxide. The microparticles were derived from silica gel (nominal pore diameter, 15-80 nm) by impregnation with a citric acid/ethanol solution and a ferric nitrate/ethanol solution and then by calcination in a nitrogen atmosphere to produce ferrimagnetic fine particles of spinel-type iron oxide (gamma-Fe(2)O(3)) inside the pore. They were characterized by X-ray diffraction. The calibration curve of the glucose sample (2 microL injected) was linear between 2.5 x 10(-6) and 5 x 10(-4) mol/L (R = 0.9995), and the detection limit was 1.0 x 10(-6) mol/L or 0.36 ng of injected glucose (S/N = 3). The repeatability for a 5 x 10(-4) mol/L glucose solution was RSD = 1.5% (n = 6). Application to the assay of glucose in a fermentation broth is illustrated. The GOx MMP were stable and active for more than eight months when kept at 10 degrees C.     

基于二氧化硅球腔阵列的葡萄糖传感器研究

在二氧化硅球腔阵列电极上,通过电沉积普鲁士蓝和直接吸附葡萄糖氧化酶,制备了一种新型葡萄糖生物传感器。该传感器对酶催化反应产物过氧化氢的选择性催化还原特性可实现对葡萄糖的检测,实验结果表明,传感器的最佳工作电位是－0．3V,测试溶液的最佳pH值为6．0。在选定的工作条件下,传感器的线性范围为2．49×10-5－2．42×10-3mol／L,检测极限值为7．2×10-6mol／L（S／N=3）,米氏常数为1．136mmol／L。该方法制备的生物传感器能有效降低干扰,具有潜在的应用价值。     

Direct determination of oxygen by HPLC. 1. Basic principles of a sensitive and selective oxygen sensor

The basic principles of a novel, versatile, sensitive, and selective oxygen-sensing assay are presented in this paper. For the first time, liquid chromatography with electrochemical detection (at the hmde) has been used for the determination of oxygen. All factors concerning optimization of the chromatographic separation conditions and electrochemical detection with respect to direct determination of oxygen even in complex biological samples are discussed. Due to the combination of a chromatographic technique with amperometric detection, a high selectivity can be achieved. A direct and linear relationship between the oxygen concentration in the sample and the reduction current was verified in a large concentration range from saturation down to trace level oxygen concentrations. The novel oxygen-sensing assay provides a much higher sensitivity compared to conventional oxygen sensors. In principle, O(2) concentrations down to 4.5 × 10(-)(9) mol L(-)(1) O(2) (corresponding to a signal-to-noise ratio of 3) can be detected. Precision was determined by repeated measurements (n = 6) of air-saturated solutions (2.5 × 10(-)(4) mol L(-)(1) O(2), 20 °C, 920 mbar) which yielded relative standard deviations of lower than 0.2%.     

A highly selective lead-sensitive electrode with solid contact based on ionic liquid

A new polyvinylchloride membrane sensor for Pb(2+) with solid contact based on ionic liquid has been prepared. The electrode shows a Nernstian response for lead ions over a wide concentration range (1×10(-8) to 1×10(-1) mol L(-1)) and the slope of 29.8 mV/decade. The limit of detection is 4.3×10(-9) mol L(-1). It has a fast response time of 5-7 s and can be used for 4 months without any divergence in potential. The proposed sensor is not pH sensitive in the range 3.5-7.3 and shows a very good discriminating ability towards Pb(2+) ion in comparison with some alkali, alkaline earth, transition and heavy metal ions. It was successfully applied as an indicator electrode in potentiometric titration of lead ions with K(2)CrO(4) and for direct determination of Pb(2+) ions in real sample solution.     

Graphite-Poly(tetrafluoroethylene) Composite Enzyme Electrodes as Suitable Biosensors in Predominantly Nonaqueous Media

The performance of a graphite-poly(tetrafluoroethylene) Teflon composite amperometric ferrocyanide-mediated peroxidase electrode in a predominantly nonaqueous medium such as reversed micelles is discussed and compared with the behavior in a medium formed by acetonitrile/water. The composite electrode was constructed by purely physical entrapment of both the enzyme and the mediator into the bulk of the graphite-Teflon matrix with no need of covalent attachments. This biosensor responded rapidly to the changes in the concentration of both hydrogen peroxide and 2-butanone peroxide in reversed micelles formed with ethyl acetate, 0.1 mol L(-)(1) dioctyl sulfosuccinate as the surfactant, and a 4% phosphate buffer (pH 7.4) as the dispersed phase. The electrode showed a long-term operation due to the renewability of its surface. Moreover, reproducible responses were obtained with different electrodes fabricated from different composite matrixes. No significant loss of the enzyme activity was observed after four months of dry storage at 4 °C of the composite electrode. Limits of detection of 2.1 × 10(-)(7) and 3.5 × 10(-)(7) mol L(-)(1) were obtained for H(2)O(2) and 2-butanone peroxide, respectively. The possibility of using this biocomposite electrode in flowing systems, using the reversed micelles as the carrier, has been demonstrated. The kinetic of the enzymatic reaction was faster in a 90:10 acetonitrile/phosphate buffer medium than in reversed micelles, which can be attributed to the higher water content present in the former medium. A similar stability of the biosensor and a slightly better sensitivity for peroxides was observed in the acetonitrile/water mixture when compared with reversed micelles. Finally, the electrode also performed well in the flow injection mode.     

Cyclic voltammetric detection in capillary electrophoresis with application to metal ions

Fast cyclic voltammetry (CV) was evaluated over sweep rates of 20-1000 V/s at Au disk electrodes (25 and 10 μm) for end-capillary detection in capillary electrophoresis with metal ions as test analytes; some studies were also done with 25-μm Pt disk electrodes. The waveform applied to the electrode consisted of a preconcentration period (55-330 ms) followed by cyclic voltammetry (2-100 ms). Maximum signal-to-noise was obtained with the integrated CV current as the analytical signal, and this was linearly proportional to sweep rate; maximum response was obtained at sweep rates of >100 V/s for 10-μm electrodes and >200 V/s for 25-μm electrodes; sweep rates of >400 V/s caused peak tailing due to trapping of the analyte at the electrode. With this CV detection approach, comigrating analytes could be identified and determined. Reproducibilities for six analytes over the range 1.0 × 10(-)(7)-1.0 × 10(-)(5) mol/L were 2%-5%, and calibration curves were linear, with response factors in the range of 2%-6%. Detection limits (2 × peak-to-peak baseline noise) were in the range of 5 × 10(-)(9)-4 × 10(-)(8) mol/L, which are 1-2 orders of magnitude better than results obtained previously with square-wave pulsed amperometric detection of metal ions.     

Direct determination of oxygen by HPLC. 2. Chamber and sample application system for determination of o(2) at trace levels

All oxygen measurement systems so far available are characterized by a lack of suitable precision and/or required limit of detection, which would be essential for a great variety of applications. In this paper, a novel oxygen chamber together with a completely new concept of sample application ("two-chamber-siphon technique") is presented which can be used in combination with the previously reported chromatographic oxygen sensor (part 1). This new oxygen-sensing assay exhibits several advantages in comparison to conventional oxygen measurement systems: e.g., the uncontrollable influence of the surrounding atmosphere as well as oxygen consumption and storage processes are excluded. For the first time, measurements of molecular oxygen below 1 × 10(-)(7) mol L(-)(1) can be performed. Reliable quantification of oxygen in liquids and also in gaseous and solid samples can be achieved with utmost sensitivity (LOD 4.9 × 10(-)(9) mol L(-)(1) O(2) = 98 fmol of oxygen on column) and precision (RSD = 0.7%, n = 8).     

复合半导体光催化材料ZnFe2O4-TiO2/SiO2结构与光响应性能研究

采用溶胶．凝胶法制备了负载型复合半导体光催化材料ZnFe2O4-TiO2／SiO2，并通过DTA-TG、XRD、XPS、Raman、TPR及UV-Vis DRS等实验技术对复合材料的晶体结构、表面组成及光响应性能进行了表征和评价．结果表明：ZnFe2O4晶相以高分散状态存在于光催化材料的表面；ZnFe2O4与TiO2复合可使部分Fe^3＋进入体相TiO2的晶格中，促进其由锐钛矿向金红石的相转变，同时表面剩余的少量Zn计聚集形成ZnO物相；TiO2的相变由体相开始，随着ZnFe2O4含量的增加逐渐向表面扩展；SiO2的加入使活性组分更加分散，TiO2平均粒径〈10nm；ZnFe2O4的加入明显拓宽了TiO2的吸光域，并增强了对可见光的吸收．     

Ion-Pair Extraction of Metalloporphyrins into Acetonitrile for Determination of Copper(II)

Equilibrium study of ion-pair extraction of a cationic water-soluble porphyrin [5,10,15,20-tetrakis(1-methylpyridinium-4-yl)porphyrin, H(2)tmpyp(4+)] and its metalloporphyrins (MP) into the acetonitrile layer, separated by addition of sodium chloride (4.00 mol dm(-)(3)) to a 1:1 (v/v) acetonitrile-water mixed solvent, was carried out to develop a new and useful method for the determination of a subnanogram amount of copper(II). M denotes Zn(2+), Cu(2+), Co(3+), Fe(3+), and Mn(3+), and P(2)(-) is porphyrinate ion. The extraction and dissociation constants of the ion-pair complexes, defined by K(ex) = [MP(ClO(4))(4)](org)[MP(4+)](aq)(-)(1)[ClO(4)(-)](aq)(-)(4), K(dis,1) = [MP(ClO(4))(3)(+)](org)[ClO(4)(-)](org)[MP(ClO(4))(4)](org)(-)(1), and K(dis,2) = [MP(ClO(4))(2)(2+)](org)[ClO(4)(-)](org)[MP(ClO(4))(3)(+)](org)(-)(1), were determined by taking into account the partition constant of sodium perchlorate (K(D) = 1.82 ± 0.01). The equilibrium constants were found to be K(ex)K(dis,1) = (7.2 ± 1.3) × 10(4), (6.4 ± 0.9) × 10(4), (1.35 ± 0.13) × 10(5), (4.8 ± 0.6) × 10(3), (1.23 ± 0.05) × 10(4), and (1.42 ± 0.07) × 10(3) at 25 °C for the free base porphyrin (H(2)tmpyp(4+)) and the metalloporphyrins of zinc(II), copper(II), cobalt(III), iron(III), and manganese(III), respectively. The K(dis,2) values were (2.9 ± 1.4) × 10(-)(2), (3.1 ± 1.1) × 10(-)(2), (8.0 ± 4.9) × 10(-)(3), and (5.1 ± 2.2) × 10(-)(2) for the free base porphyrins and the metalloporphyrins of zinc(II), copper(II), and cobalt(III), respectively. The results were developed for determination of a trace amount of copper(II) (3 × 10(-)(8)-4 × 10(-)(6) mol dm(-)(3)) in natural water samples using H(2)tmpyp(4+) with a molar absorptivity of 3.1 × 10(5) mol(-)(1) dm(3) cm(-)(1) at a precision of 1.3% (RSD). The determination of copper(II) was not interfered by the presence of 10(-)(4) mol dm(-)(3) of Mn(2+), Co(2+), Ni(2+), Hg(2+), Cd(2+), Ag(+), Cr(3+), V(5+), Al(3+), Mg(2+), Ca(2+), Br(-), I(-), SCN(-), and S(2)O(3)(2)(-) and 10(-)(5) mol dm(-)(3) of Fe(3+), Zn(2+), and Pd(2+).     

金属—PAN—S配合物的极谱研究——Ⅱ:Fe~(3+)—PAN—S—TEA—NH_3·H_2O—NH_4Cl体系配合吸附波

在NH_3·H_2O—NH_4Cl—三乙醇胺底液中Fe(Ⅲ)与PAN—S产生一灵敏的配合吸附波,峰电位在—0.50伏(vs.SCE)。峰电位与铁离子浓度在2.8×10~8～3.4×10~(-6)mol/L范围内线性良好,检出下限可达2.8×10~(-8)mol/L。该法用于乳粉、头发、血清等样品的测定,结果满意。     

Synthesis and characterization of AuNPs-modificated Fe2O3/ZnFe2O4 heterostructures for highly sensitive 1-butanol detection

Journal of Materials Science - In this work, the Fe2O3/ZnFe2O4 heterostructures were synthesized by solvothermal and calcination decomposition methods, and then used for 1-butanol detection. The...     

Utilizing a CdTe quantum dots-enzyme hybrid system for the determination of both phenolic compounds and hydrogen peroxide

In this paper, we attempt to construct a simple and sensitive detection method for both phenolic compounds and hydrogen peroxide, with the successful combination of the unique property of quantum dots and the specificity of enzymatic reactions. In the presence of H2O2 and horseradish peroxidase, phenolic compounds can quench quantum dots' photoluminescence efficiently, and the extent of quenching is severalfold to more than 100-fold increase. Quinone intermediates produced from the enzymatic catalyzed oxidation of phenolic compounds were believed to play the main role in the photoluminescence quenching. Using a quantum dots-enzyme system, the detection limits for phenolic compounds and hydrogen peroxide were detected to be approximately 10(-7) mol L(-1). The coupling of efficient quenching of quantum dot photoluminescence by quinone and the effective enzymatic reactions make this a simple and sensitive method for phenolic compound detection and great potential in the development of H2O2 biosensors for various analytes.     

Thionine covalently tethered to multilayer horseradish peroxidase in a self-assembled monolayer as an electron-transfer mediator

A new approach to construct a reagentless enzyme biosensor is described. Based on multilayer horseradish peroxidase in a self-assembled monolayer configuration, the biosensor was constructed using multilayer thionine covalently tethered to the enzyme as an electron-transfer mediator. The multilayer enzyme and the multilayer mediator were stepwisely synthesized onto an l-cysteine-assembled gold electrode using glutaraldehyde as a bifunctional reagent. The multilayer mediator tethered to the multilayer enzyme could effectively and stably shuttle electrons between the electrode and the multilayer enzyme linked onto the monolayer. The sensitivity of the resulting enzyme biosensor with eight layers of enzyme and three layers of mediator was more than 250 μA cm(-)(2) for 1.0 × 10(-)(4) mol/L hydrogen peroxide under optimal conditions, whereas such a modified electrode with one layer of enzyme and one layer of mediator did not yield a detectable response to 1.0 × 10(-)(4) mol/L hydrogen peroxide.     

A new Schiff's base ligand immobilized agarose membrane optical sensor for selective monitoring of mercury ion

A highly selective optical sensor was developed for the Hg(2+) determination by chemical immobilization of 2-[(2-sulfanylphenyl)ethanimidoyl]phenol (L), on an agarose membrane. Spectrophotometric studies of complex formation between the Schiff's base ligand L and Hg(2+), Sr(2+), Mn(2+), Cu(2+), Al(3+), Cd(2+), Zn(2+), Co(2+) and Ag(+) metal ions in methanol solution indicated a substantially larger stability constant for the mercury ion complex. Consequently, the Schiff's base L was used as an appropriate ionophore for the preparation of a selective Hg(2+) optical sensor, by its immobilization on a transparent agarose film. A distinct color change, from yellow to green-blue, was observed by contacting the sensing membrane with Hg(2+) ions at pH 4.5. The effects of pH, ionophore concentration, ionic strength and reaction time on the immobilization of L were studied. A linear relationship was observed between the membrane absorbance at 650 nm and Hg(2+) concentrations in a range from 1×10(-2) to 1×10(-5) mol L(-1) with a detection limit (3σ) of 1×10(-6) mol L(-1). No significant interference from 100 times concentrations of a number of potentially interfering ions was detected for the mercury ion determination. The optical sensor was successfully applied to the determination of mercury in amalgam alloy and spiked water samples.     

Fabrication of a glucose biosensor based on citric acid assisted cobalt ferrite magnetic nanoparticles

A novel and practical glucose biosensor was fabricated with immobilization of Glucose oxidase (GOx) enzyme on the surface of citric acid (CA) assisted cobalt ferrite (CF) magnetic nanoparticles (MNPs). This innovative sensor was constructed with glassy carbon electrode which is represented as (GOx)/CA-CF/(GCE). An explicit high negative zeta potential value (-22.4 mV at pH 7.0) was observed on the surface of CA-CF MNPs. Our sensor works on the principle of detection of H2O2 which is produced by the enzymatic oxidation of glucose to gluconic acid. This sensor has tremendous potential for application in glucose biosensing due to the higher sensitivity 2.5 microA/cm2-mM and substantial increment of the anodic peak current from 0.2 microA to 10.5 microA.     

Electrochemiluminescent detection based on solid-phase extraction at tris(2,2'-bipyridyl)ruthenium(II)-modified ceramic carbon electrode

A sensitive electrochemiluminescent detection scheme by solid-phase extraction at Ru(bpy)3(2+)-modified ceramic carbon electrodes (CCEs) was developed. The as-prepared Ru(bpy)3(2+)-modified CCEs show much better long-term stability than other Nafion-based Ru(bpy)3(2+)-modified electrodes and enjoy the inherent advantages of CCEs. The log-log calibration plot for dioxopromethazine is linear from 1.0 x 10(-9) to 1.0 x 10(-4) mol L(-1) using the new detection scheme. The detection limit is 6.6 x 10(-10) mol L(-1) at a signal-to-noise ratio of 3. The new scheme improves the sensitivity by approximately 3 orders of magnitude, which is the most sensitive Ru(bpy)3(2+) ECL method. The scheme allows the detection of dioxopromethazine in a urine sample within 3 min. Since Ru(bpy)3(2+) ECL is a powerful technique for determination of numerous amine-containing substances, the new detection scheme holds great promise in measurement of free concentrations, investigation of protein-drug interactions and DNA-drug interactions, pharmaceutical analysis, and so on.     

Interactions of vitamin K3 with herring-sperm DNA using spectroscopy and electrochemistry

By means of ultraviolet-visible (UV-Vis) and fluorescence spectra, the binding ratio between vitamin K(3) and herring-sperm DNA in a physiological pH environment (pH = 7.40) was determined as n(K3):n(DNA) = 2:1, and the binding constants of vitamin K(3) binding to DNA at different temperatures were determined as K(θ)(298K) = 1.28 × 10(5) L·mol(-1) and K(θ)(310K) = 7.19 × 10(4) L·mol(-1), which were confirmed using the double reciprocal method are Δ(r)H(m)(θ) = -3.57 × 10(4) J·mol(-1), Δ(r)G(m)(θ) = -2.92 × 10(4) J·mol(-1), and Δ(r)S(m)(θ) = 217.67 J·mol(-1)K(-1). The driving power of this process was enthalpy. An intercalation binding of the vitamin K(3) with DNA was supported by a competitive experiment using acridine orange (AO) as a spectral probe. By combination analysis of the Scatchard method and cyclic voltammetry, we suggested that the interaction mode between vitamin K(3) and herring-sperm DNA would be a mixed mode. The quinonoid, duality fused-ring of vitamin K(3) can intercalate into the base pairs of DNA, and there is an electrostatic binding along with intercalation binding.     

Electron-transfer reactivity and enzymatic activity of hemoglobin in a SP Sephadex membrane

Hemoglobin can exhibit a direct electron-transfer reaction after being entrapped in a SP Sephadex membrane. A pair of stable and well-defined redox waves are obtained at a hemoglobin-SP sephadex modified pyrolytic graphite electrode. The anodic and cathodic peak potentials are located at -0.244 and -0.336 V (vs SCE), respectively. On the other hand, the peroxidase activity of the protein in the membrane is also greatly enhanced. The apparent Michaelis-Menten constant is calculated to be 1.9 mM, which shows a large catalytic activity of hemoglobin in the SP Sephadex membrane toward hydrogen peroxide (H2O2). According to the direct electron-transfer property and enhanced peroxidase activity of Hb in the membrane, a Hb/SP Sephadex membrane-based H2O2 biosensor is prepared, with a linear range approximately 5.0 x 10(-6) to 1.6 x 10(-4) mol/L.     

On-column coaxial flow chemiluminescence detection for underivatized amino acids by pressurized capillary electrochromatography using a monolithic column

A new method for pressurized capillary electrochromatography (pCEC) coupling with chemiluminescence (CL) detection using a modified on-column coaxial flow detection interface was developed. To evaluate the feasibility and reliability of the experimental setup, the typical CL compounds luminol and isoluminol were separated and detected by using this pCEC-CL system. A detailed investigation of CL detection interface and postcolumn CL reagent flow rate parameters was described. The excellent resolution and detection sensitivity was achieved by using 3-microm ODS-C18 packed column with 30% ACN (v/v), 5 mmol/L phosphate buffer (pH 8.0). Moreover, with the presence of Co(II) (1.0 x 10(-4) mol/L) in the mobile phase, the linear range of the concentration for luminol was 2.0 x 10(-9)-2.0 x 10(-6) mol/L with a detection limit (S/N = 3) of 2.0 x 10(-10) mol/L, and 2.5 x 10(4) theoretical plates was achieved. In addition, separation and detection of the underivatized amino acids (l-threonine and l-tyrosine) were accomplished by using a polymerized monolithic column based on the principle of the luminol-H2O2-Cu(II)-amino acid CL system. Under the optimum conditions, the mixture of amino acids was efficiently separated with satisfactory results.