Construction of an Amperometric Glucose Biosensor by Immobilization of Glucose Oxidase on Nanocomposite at the Surface of FTO Electrode

Fluorine? tin oxide (FTO) nanostructure was developed on the surface of a glass plate using spray payroliziz method. A new electrochemical biosensor was fabricated based on a layer by layer process. In this process chitosan? Fe₃O₄ (CH? Fe₃O₄) nanocomposite film was prepared at the surface of FTO electrode by dip? coating method. In the next step, the glucose oxidase (GOx) was immobilized on the CH? Fe₃O₄/FTO nanocomposite electrode. The GOx/CH? Fe₃O₄/FTO bioelectrode has a linear range of 10–270 µM and a detection limit of 5 µM. The highest sensitivity was obtained at 1.2 µA mM^?1 cm^?2.     

General Preparation of Heme Protein Functional Fe3O4@Au‐Nps Magnetic Nanocomposite for Sensitive Detection of Hydrogen Peroxide

Stable magnetic nanocomposite of gold nanoparticles (Au‐NPs) decorating Fe₃O₄ core was successfully synthesized by the linker of Boc‐L‐cysteine. Transmission electron microscope (TEM), energy dispersive X‐ray spectroscopy (EDX) and cyclic voltammograms (CV) were performed to characterize the as‐prepared Fe₃O₄@Au‐Nps. The results indicated that Au‐Nps dispersed homogeneously around Fe₃O₄ with the ratio of Au to Fe₃O₄ nanoparticles as 5–10/1 and the apparent electrochemical area as 0.121 cm². After self‐assembly of hemoglobin (Hb) on Fe₃O₄@Au‐Nps by electrostatic interaction, a hydrogen peroxide biosensor was developed. The Fe₃O₄@Au‐Nps/Hb modified GCE exhibited fast direct electron transfer between heme center and electrode surface with the heterogeneous electron transfer rate constant (Ks ) of 3.35 s⁻¹. Importantly, it showed excellent electrocatalytic activity towards hydrogen peroxide reduction with low detection limit of 0.133 μM (S /D =3) and high sensitivity of 0.163 μA μM⁻¹, respectively. At the concentration evaluated, the interfering species of glucose, dopamine, uric acid and ascorbic acid did not affect the determination of hydrogen peroxide. These results demonstrated that the introduction of Au‐Nps on Fe₃O₄ not only stabilized the immobilized enzyme but also provided large surface area, fast electron transfer and excellent biocompatibility. This facile nanoassembly protocol can be extended to immobilize various enzymes, proteins and biomolecules to develop robust biosensors.     

Direct Electrochemistry of Hemoglobin Based on Fe3O4@SiO2 Nanoparticles Modified Electrode

A biosensor based on hemoglobin‐Fe₃O₄@SiO₂ nanoparticle bioconjunctions modified indium‐tin‐oxide (Hb/Fe₃O₄@SiO₂/ITO) electrode was fabricated to determine the concentration of H₂O₂. UV‐vis absorption spectra, fourier transform infrared (FT‐IR) spectroscopy, cyclic voltammetry (CV) and high‐resolution transmission electron microscopy (HRTEM) were used to characterize the bioconjunction of Fe₃O₄@SiO₂ with Hb. Experimental results demonstrate that the immobilized Hb on the Fe₃O₄@SiO₂ matrix retained its native structure well. In addition, Fe₃O₄@SiO₂ nanoparticles (NPs) are very effective in facilitating electron transfer of the immobilized enzyme, which can be attributed to the unique nanostructure and larger surface area of the Fe₃O₄@SiO₂ NPs. The biosensor displayed good performance for the detection of H₂O₂ with a wide linear range from 2.03×10^?6 to 4.05×10^?3 mol/L and a detection limit of 0.32 µmol/L. The resulting biosensor exhibited fast amperometric response, good stability, reproducibility, and selectivity to H₂O₂.     

Disposable Amperometric Biosensor Based on Poly‐L‐lysine and Fe3O4 NPs‐chitosan Composite for the Detection of Tyramine in Cheese

An amperometric tyramine biosensor based on poly‐L‐lysine (PLL) and Fe₃O₄ nanoparticles (Fe₃O₄NP) modified screen printed carbon electrode (SPCE) was developed. PLL was formed on the SPCE by the electropolymerization of L‐lysine. Subsequently, Fe₃O₄NP suspension prepared in chitosan (CH) solution was casted onto the PLL/SPCE. Tyrosinase (Ty) enzyme was immobilized onto the modified Fe₃O₄?CH/PLL/SPCE and the electrode was coated with Nafion to fabricate the Ty/Fe₃O₄?CH/PLL/SPCE. Different techniques including scanning electron microscopy, chronoamperometry (i–t curve), cyclic voltammetry and electrochemical impedance spectroscopy were utilized to study the fabrication processes, electrochemical characteristics and performance parameters of the biosensor. The analytical performance of the tyramine biosensor was evaluated with respect to linear range, sensitivity, limit of detection, repeatability and reproducibility. The response of the biosensor to tyramine was linear between 4.9×10^?7–6.3×10^?5 M with a detection limit of 7.5×10^?8 M and sensitivity of 71.36 μA mM^?1 (595 μA mM^?1 cm^?2). The application of the developed biosensor for the determination of tyramine was successfully tested in cheese sample and mean analytical recovery of added tyramine in cheese extract was calculated as 101.2±2.1 %. The presented tyramine biosensor is a promising approach for tyramine analysis in real samples due to its high sensitivity, rapid response and easy fabrication.     

Amperometric Ethanol Biosensor Based on Carbon Nanotubes Dispersed in Sol–Gel‐Derived Titania–Nafion Composite Film

Composite solution of sol–gel‐derived titania and perfluorosulfonated ionomer (Nafion) was used as a solubilizing agent for multiwalled carbon nanotubes (CNT) as well as an encapsulation matrix for alcohol dehydrogenase (ADH) for the fabrication of a highly sensitive and stable amperometric ethanol biosensor. ADH was immobilized within a thin film of CNT–titania–Nafion composite film coated on a glassy carbon electrode. Because of the mesoporous nature of the CNT–titania–Nafion composite film, the present biosensor exhibited remarkably fast response time within 2 s. The presence of CNT in the composite film increases not only the sensitivity of the ethanol biosensor but also the long‐term stability of the biosensor. The present biosensor responds linearly to ethanol in the wide concentration ranges from 1.0×10^?5 M to 3.0×10^?3 M with the sensitivity of 51.6 mA M^?1cm^?2. The present biosensor showed good long‐term stability with 75% of its activity retained after 4 weeks of storage in 50 mM phosphate buffer at pH 7.0.     

Hydrogen peroxide biosensor based on the immobilization of horseradish peroxidase on ��-Al2O3 nanoparticles/chitosan film-modified electrode

An amperometric biosensor based on horseradish peroxidase (HRP) and ??-Al₂O₃/chitosan composite film at a glassy carbon electrode has been developed. Hydrogen peroxide (H₂O₂) was detected with the aid of ferrocene monocarboxylic acid mediator to transfer electrons between the electrode and HRP. The morphology and composition of the modified electrode were characterized by scanning electron microscopy and electrochemical impedance spectroscopy. The electrochemical characteristics of the biosensor were studied by cyclic voltammetry and amperometry. The effects of HRP concentration, the applied potential, and the pH values of the buffer solution on the response of the sensor were investigated for optimum analytical performance. The proposed biosensor showed high sensitivity (0.249?A M^?1?cm^?2) and a fast response (<5?s) to H₂O₂ with the detection limit of 0.07???M. The linear response range of the enzyme electrode to H₂O₂ concentration was from 0.5 to 700???M with a correlation coefficient of 0.9998. The apparent Michaelis-Menten constant of the biosensor was calculated to be 0.818?mM, exhibiting a high enzymatic activity and affinity for H₂O₂.     

Detection of Dexamethasone Sodium Phosphate in Blood Plasma: Application of Hematite in Electrochemical Sensors

We studied sensor application of a graphene oxide and hematite (α‐Fe₂O₃/GO) composite electrode well‐characterized by the SEM and XRD. Through differential pulse voltammetry (DPV), oxidation of dexamethasone sodium phosphate (DSP) was studied at the surface of a glassy carbon electrode (GCE) modified with graphene oxide nanosheets (GO) and the α‐Fe₂O₃/GO composite. The values of the transfer coefficient (α) and the diffusion coefficient (D) of DSP were 0.5961 and 4.71×10^?5 cm² s^?1 respectively. In the linear range of 0.1–50 μM, the detection limit (DL) was 0.076 μM. In the second step, a GCE was modified with α‐Fe₂O₃/GO composite and the DSP measurement step was repeated to analyzed and compare the effects of hematite nanoparticles present on graphene oxide surfaces. According to the results, α and D were 0.52 and 2.406×10^?4 cm² s^?1 respectively and the DL was 0.046 μM in the linear range of 0.1–10.0 μM. The sensor is simple, inexpensive and uses blood serum.     

Enhanced NADH Oxidation Using Polytyramine/Carbon Nanotube Modified Electrodes for Ethanol Biosensing

Polytyramine (PT) has been electro‐deposited onto multi‐walled carbon nanotube (MWCNT) modified glassy carbon (GC) electrodes via oxidation of tyramine in 0.1 M H₃PO₄ by cycling the potential over the range of −400 mV to 1300 mV (versus Ag/AgCl). The reactivity of the resulting chemically‐modified electrodes was characterized using cyclic voltammetry in the presence and absence of reduced nicotinamide adenine dinucleotide (NADH). The modified electrodes displayed electrochemical activity due to the formation of quinone species and were catalytically active towards NADH oxidation by lowering the oxidation peak potential by 170 mV compared to the value of the MWCNT modified electrode with a peak potential of 180±10 mV (versus Ag/AgCl). The MWCNT/PT surface was further characterized using SEM and XPS methods, which indicated that a thin polymeric film had been formed on the electrode surface. The present work demonstrates the advantage of using PT as a platform that combines both the immobilization of alcohol dehydrogenase (ADH) and the mediation of NADH oxidation at a low overpotential essential to the design of high performance ethanol biosensors, all within an easily electropolymerizable film. The resulting biosensor displayed an ethanol sensitivity of 4.28±0.06 μA mM⁻¹ cm⁻², a linear range between 0.1 mM and 0.5 mM and a detection limit of 10 μM.     

Synthesis of orientedly bioconjugated core/shell Fe3O4@Au magnetic nanoparticles for cell separation

Orientedly bioconjugated core/shell Fe₃O₄@Au magnetic nanoparticles were synthesized for cell separation. The Fe₃O₄@Au magnetic nanoparticles were synthesized by reducing HAuCl₄ on the surfaces of Fe₃O₄ nanoparticles, which were further characterized in detail by TEM, XRD and UV-vis spectra. Anti-CD3 monoclonal antibody was orientedly bioconjugated to the surface of Fe₃O₄@Au nanoparticles through affinity binding between the Fc portion of the antibody and protein A that covalently immobilized on the nanoparticles. The oriented immobilization method was performed to compare its efficiency for cell separation with the non-oriented one, in which the antibody was directly immobilized onto the carboxylated nanoparticle surface. Results showed that the orientedly bioconjugated Fe₃O₄@Au MNPs successfully pulled down CD3⁺ T cells from the whole splenocytes with high efficiency of up to 98.4%, showing a more effective cell-capture nanostructure than that obtained by non-oriented strategy. This developed strategy for the synthesis and oriented bioconjugation of Fe₃O₄@Au MNPs provides an efficient tool for cell separation, and may be further applied to various fields of bioanalytical chemistry for diagnosis, affinity extraction and biosensor.     

Preparation of an Electrode Modified with an Electropolymerized Film as a Mediator of NADH Oxidation and Its Application in an Ethanol/O2 Biofuel Cell

This paper reports a novel mediator for the oxidation of β‐nicotinamide adenine dinucleotide (NAD⁺/NADH), an electropolymeric film (pAPRu) of [Ru(NH₂‐phen)₃]²⁺. A pAPRu‐modified electrode was prepared via electropolymerization and exhibited catalytic activity toward the electrochemical oxidation of NADH due to the imine moieties of pAPRu. The electrochemical oxidation of ethanol was observed using an alcohol dehydrogenase (ADH)‐immobilized electrode. A compartmentless ethanol/O₂ biofuel cell composed of an ADH anode and a bilirubin oxidase cathode was constructed. The maximum current density and the maximum power density of the biofuel cell were 190 µA cm^?2 and 31 µW cm^?2 (at 0.29 V), respectively.     

Reduced Graphene Oxide|Carbon Ceramic Electrode Modified with CdS‐Hemoglobin as a Sensitive Hydrogen Peroxide Biosensor

A sensitive hydrogen peroxide (H₂O₂) biosensor was developed based on a reduced graphene oxide|carbon ceramic electrode (RGO|CCE) modified with cadmium sulfide‐hemoglobin (CdS‐Hb). The electron transfer kinetics of Hb were promoted due to the synergetic function of RGO and CdS nanoparticles. The transfer coefficient (α) and the heterogeneous electron transfer rate constant (k_s) were calculated to be 0.54 and 2.6 s^?1, respectively, indicating a great facilitation achieved in the electron transfer between Hb and the electrode surface. The biosensor showed a good linear response to the reduction of H₂O₂ over the concentration range of 2–240 µM with a detection limit of 0.24 µM (S/N=3) and a sensitivity of 1.056 µA µM^?1 cm^?2. The high surface coverage of the CdS‐Hb modified RGO|CCE (1.04×10^?8 mol cm^?2) and a smaller value of the apparent Michaelis? Menten constant (0.24 mM) confirmed excellent loading of Hb and high affinity of the biosensor for hydrogen peroxide.     

Effect of Enzyme and Cofactor Immobilization on the Response of Ethanol Oxidation in Zirconium Phosphate Modified Biosensors

Two different self‐contained ethanol amperometric biosensors incorporating layered [Ru(phend)₂bpy]²⁺‐intercalated zirconium phosphate (ZrP) as the mediator as well as yeast‐alcohol dehydrogenase (y‐ADH) and its cofactor nicotinamide adenine dinucleotide (NAD⁺) were constructed to improve upon a design previously reported where only this mediator was immobilized in the surface of a modified electrode. In the first biosensor, a [Ru(phend)₂bpy]²⁺‐intercalated ZrP modified carbon paste electrode (CPE) was improved by immobilizing in its surface both y‐ADH and NAD⁺ using quaternized Nafion membrane. In the second biosensor, a glassy carbon electrode was modified with [Ru(phend)₂bpy]²⁺‐intercalated ZrP, y‐ADH, and NAD⁺ using Nafion as the holding matrix. Calibration plots for ethanol sensing were constructed in the presence and absence of ZrP. In the absence of ZrP in the surface of the modified glassy carbon electrode, leaching of ADH was observed as detected by UV‐vis spectrophotometry. Ethanol sensing was also tested in the presence and absence of ascorbate to measure the selectivity of the sensor for ethanol. These two ethanol biosensors were compared to a previously reported one where the y‐ADH and the NAD⁺ were in solution, not immobilized.     

A Sensitive Electrochemical Sensor Based on Graphene Oxide Nanosheets Decorated by Fe3O4@Au Nanostructure Stabilized on Polypyrrole for Efficient Triclosan Sensing

Triclosan is broadly utilized as preservative or antiseptic in various cosmetic and personal care products. It becomes hazardous for environmental safety and human health more than a certain concentration. In this research, graphene oxide (GO) nanosheets were prepared by composing Fe₃O₄@Au nanostructure decorated GO together with polypyrrole (PPy) (Fe₃O₄@Au‐PPy/GO nanocomposite) in a facile way. The composite excellent increased the electrochemical response, presenting a high sensitive electrochemical method for triclosan detection. The synthesized Fe₃O₄@Au‐PPy/GO nanocomposite was characterized for its morphological, magnetically and structural properties by FESEM‐mapping, TEM, and XRD. The Fe₃O₄@Au‐PPy/GO nanocomposites modified glassy carbon electrodes (GCE), Fe₃O₄@Au‐PPy/GO GCE, showed a higher sensitivity good stability, reproducibility, lower LOD (2.5×10^?9 M) and potential practical application in electrochemical detection of triclosan under optimized experimental conditions.     

Amperometric Biosensor for Hydrogen Peroxide Based on Myoglobin Doped Multiwalled Carbon Nanotube Enhanced Grafted Collagen Matrix

Abstract

A reagentless H₂O₂ sensor based on the direct electron transfer of myoglobin (Mb) doped in multiwalled carbon nanotubes enhanced grafted collagen matrix is proposed. The formal potential of the immobilized Mb was ?0.358 V with a surface coverage of 4.0×10^?10 mol cm^?2. The electrode process was surface‐controlled with an electron transfer rate constant of 9.7 s^?1. The proposed biosensor displayed an excellent electrocatalytic response to the reduction of H₂O₂ with a linear range from 0.6 to 39.0 µM. Owing to the good biocompatibility and high enzyme loading of the matrix the biosensor exhibited acceptable stability and reproducibility.     

Preparation,Characterization and Electrochemical Application of Graphene‐metallic Nanocomposites

Three different Graphene‐Metallic (Graphene‐Me) nanocomposites – Graphene‐Silver (Graphene‐Ag), Graphene‐Gold (Graphene‐Au) and Graphene‐Platinum (Graphene‐Pt) nanocomposites – were prepared and characterized. The electrochemical performances of these nanocomposites were tested by incorporating them with glassy carbon paste electrode (GCPE) and used them in biofuel cells (BFC) and as amperometric xanthine biosensor transducers. Present work contains the first application of Graphene‐Au and Graphene‐Ag nanocomposite in BFCs and also first application of these Graphene‐Me nanocomposites in xanthine biosensors. Considering BFC, power and current densities were calculated as 2.03 µW cm^?2 and 167.46 µA cm^?2 for the plain BFC, 3.39 µW cm^?2 and 182.53 µA cm^?2 for Graphene‐Ag, 4.43 µW cm^?2 and 230.15 µA cm^?2 for Grapehene‐Au and 6.23 µW cm^?2 and 295.23 µA cm^?2 for Graphene‐Pt nanocomposite included BFCs respectively. For the amperometric xanthine biosensor linear ranges were obtained in the concentration range between 5 µM and 50 µM with the RSD (n=3 for 30 µM xanthine) value of 4.28 % for plain xanthine biosensor, 3 µM and 50 µM with the RSD (n=3 for 30 µM xanthine) value of 9.37 % for Graphene‐Ag, 5 µM to 20 µM with the RSD (n=3 for 5 µM xanthine) value of 9.00 % and 30 µM to 70 µM with the RSD (n=3 for 30 µM xanthine) value of 8.80 % for Grapehene‐Au and 1 µM and 70 with the the RSD (n=3 for 30 µM xanthine) value of 2.59 % for Grapehene‐Pt based xanthine biosensors respectively.     

Hemoglobin‐Titanate Composite Based Biosensor for the Amperometric Determination of Hydrogen Peroxide in Acidic Medium

A hemoglobin‐titanate composite based biosensor was chosen for determination of H₂O₂ in an acidic medium. CV results of the Hb‐titanate modified pyrolytic graphite electrode showed a pair of well‐defined, quasi‐reversible redox peaks centered at ?246 mV (vs. Ag/AgCl) in a pH 5.0 HAc‐NaAc buffer solution. The modified electrode exhibited good electrocatalytic response for monitoring H₂O₂ and had a large linear detection range from 20 μM to 3.2 mM with a detection limit of 8 μM (S/N=3) and a sensitivity of 29.7 mA M^?1 cm^?2 in the pH 5.0 solution. The biosensor also possessed good long term storage stability.     

Enrichment and Identification of Metallothionein by Functionalized Nano-Magnetic Particles and Matrix Assisted Laser Desorption Ionization Time-of-Flight Mass Spectrometry

As a low molecular weight protein with the ability of binding metal ions and high inducibility, metallothionein (MT) is often regarded as an important biomarker for assessment of heavy metal pollution in water environment. In the light of that the traditional process of enrichment and identification is time-consuming and complicated, we prepared a core-shell nanoparticle, gold-coated iron oxide nanoparticles (Fe₃O₄@Au NPs) herein. It possessed the advantages of fast response to magnetic fields and optical properties attributing to Fe₃O₄ and Au nanoparticles, respectively. The Fe₃O₄@Au nanoparticles could be used to enrich MT simply through Au–S interaction, and the purified proteins were determined by matrix assisted laser desorption ionization time-of-flight mass spectrometry (MALDI-TOF/MS). The results showed that the Fe₃O₄@Au nanoparticles could directly enrich MT from complex solutions and the detection limit could be as low as 10 fg mL^?1.     

Direct Electron Transfer and Electrocatalysis of Myoglobin Based on its Direct Immobilization on Carbon Ionic Liquid Electrode

Direct electron transfer of myoglobin (Mb) was achieved by its direct immobilization on carbon ionic liquid electrode (CILE) with a conductive hydrophobic ionic liquid, 1‐butyl pyridinium hexaflourophosphate ([BuPy][PF₆]) as binder for the first time. A pair of well‐defined, quasi‐reversible redox peaks was observed for Mb/CILE resulting from Mb redox of heme Fe(III)/Fe(II) redox couple in 0.1 M phosphate buffer solution (pH 7.0) with oxidation potential of ?0.277 V, reduction potential of ?0.388 V, the formal potential E°′ (E°′=(E_pa+E_pc)/2) at ?0.332 V and the peak‐to‐peak potential separation of 0.111 V at 0.5 V/s. The average surface coverage of the electroactive Mb immobilized on the electrode surface was calculated as 1.06±0.03×10^?9 mol cm^?2. Mb retained its bioactivity on modified electrode and showed excellent electrocatalytic activity towards the reduction of H₂O₂. The cathodic peak current of Mb was linear to H₂O₂ concentration in the range from 6.0 μM to 160 μM with a detection limit of 2.0 μM (S/N=3). The apparent Michaelis–Menten constant (K and the electron transfer rate constant (k_s) were estimated to be 140±1 μM and 2.8±0.1 s^?1, respectively. The biosensor achieved the direct electrochemistry of Mb on CILE without the help of any supporting film or any electron mediator.     

A Novel Biomimetic Hydrogen Peroxide Biosensor Based on Pt Flowers‐decorated Fe3O4/Graphene Nanocomposite

A sensitive and selective amperometric H₂O₂ biosensor was obtained by utilizing the electrodeposition of Pt flowers on iron oxide‐reduced graphene oxide (Fe₃O₄/rGO) nanocomposite modified glassy carbon electrode (GCE). The morphology of Fe₃O₄/rGO and Pt/Fe₃O₄/rGO was characterized by transmission electron microscopy (TEM) and scanning electron microscopy (SEM), respectively. The step‐wise modification and the electrochemical characteristics of the resulting biosensor were characterized by cyclic voltammetry (CV) and chronoamperometry methods. Thanks to the fast electron transfer at the Pt/Fe₃O₄/rGO electrode interface, the developed biosensor exhibits a fast and linear amperometric response upon H₂O₂. The linear range of Pt/Fe₃O₄/rGO is 0.1∼2.4 mM (R²=0.998), with a sensitivity of 6.875 μA/mM and a detection limit of 1.58 μM (S/N=3). In addition, the prepared biosensor also provides good anti‐interferent ability and long‐term stability due to the favorable biocompatibility of the electrode interface. The proposed sensor will become a reliable and effective tool for monitoring and sensing the H₂O₂ in complicate environment.