The authors describe enzyme based nanobiosensors for continuous monitoring of glucose, with the long term goal of using them as smart diagnostic tattoos. The method is founded on two main features: (1) The fluorescence intensity and decay times of glucose oxidase (GOx) and of GOx labeled with fluorescein (FS) or a ruthenium chelate (Ru) reversibly change during interaction with glucose; (2) The (labeled) enzyme is linked to magnetite magnetic nanoparticles (MNPs) which permits the MNPs to be physically manipulated. It is found that a stable link between MNPs and GOx is only accomplished if the number of amino groups on the GOX is artificially enlarged (to form GOxsam). Fluorescence decay data are best acquired with 8-nm MNPs where scattering is marginal; The activity of GOx is found not to be affected by immobilization on the MNPs. The various immobilized enzymes (GOxsam, GOxsam-FS and GOxsam-Ru; all on MNPs) differ only slightly in terms of linear response to glucose which ranged from 0.5 mM to at least 3.5 mM. The RSDs are about 5% (for n = 5), the detection limits are at ~50 μM, and the sensor lifetimes are >1 week.
Graphical abstract Nanobiosensors consisting of Fe3O4 magnetic nanoparticles linked to glucose oxidase, previously enriched with amino groups (GOxsam) and containing fluorescein (FS) or a ruthenium derivative (Ru), are presented as a new kind of smart tattoos for glucose monitoring.
We have studied the direct electrochemistry of glucose oxidase (GOx) immobilized on electrochemically fabricated graphite nanosheets (GNs) and zinc oxide nanoparticles (ZnO) that were deposited on a screen printed carbon electrode (SPCE). The GNs/ZnO composite was characterized by using scanning electron microscopy and elemental analysis. The GOx immobilized on the modified electrode shows a well-defined redox couple at a formal potential of −0.4 V. The enhanced direct electrochemistry of GOx (compared to electrodes without ZnO or without GNs) indicates a fast electron transfer at this kind of electrode, with a heterogeneous electron transfer rate constant (Ks) of 3.75 s−1. The fast electron transfer is attributed to the high conductivity and large edge plane defects of GNs and good conductivity of ZnO-NPs. The modified electrode displays a linear response to glucose in concentrations from 0.3 to 4.5 mM, and the sensitivity is 30.07 μA mM−1 cm−2. The sensor exhibits a high selectivity, good repeatability and reproducibility, and long term stability.
Graphical representation for the fabrication of GNs/ZnO composite modified SPCE and the immobilization of GOx
The authors describe a method for the preparation of orange-red emissive carbon dots (CDs) with excitation/emission peaks at 520/582 nm. The CDs were hydrothermally prepared by a one-pot strategy from trimesic acid and 4-aminoacetanilide. The fluorescence of the CDs is strongly quenched by hydrogen peroxide. The oxidation of glucose by glucose oxidase (GOx) produces H2O2 that quenches the fluorescence via static quenching. Based on this phenomenon, a fluorometric method was established for the determination of glucose. Under the optimum conditions, response is linear in the 0.5 to 100 μM glucose concentration range, with a 0.33 μM limit of detection. The method is selective for glucose over its analogues and was successfully applied to the determination of glucose in diluted human serum and in urine from diabetics and healthy individuals. Recoveries from spiked samples range from 98.7 to 102.5%.
Single-walled carbon nanotubes (SWCNT), multi-walled carbon nanotubes (MWCNT) and graphene have been tested as carbon allotropes for the modification of carbon screen-printed electrodes (CSPEs) to simultaneously determine melatonin (MT) and serotonin (5-HT). Two groups of CSPEs, both 4 mm in diameter, were explored: The first includes commercial SWCNT, MWCNT and graphene, the second includes SWCNT, MWCNT, graphene oxide nanoribbons and reduced nanoribbons that were drop casted on the electrodes. The carbon nanomaterials enhanced the electroactive area in the following order: CSPE
Carbon nanomaterials on screen-printed electrodes: smart electrochemistry for fast, simultaneous and reliable detection of serotonin the molecule of happiness and melatonin the molecule of darkness.
The authors report that carbon nitride quantum dots (CN QDs) exert a strong enhancing effect on the Cu(II)/H2O2 chemiluminescent system. Chemiluminescence (CL) intensity is enhanced by CN QDs by a factor of ~75, while other carbon nanomaterials have a much weaker effect. The possible mechanism of the effect was evaluated by recording fluorescence and CL spectra and by examining the effect of various radical scavengers. Emitting species was found to be excited-state CN QDs that produce green CL peaking at 515 nm. The new CL system was applied to the sensitive detection of H2O2 and glucose (via glucose oxidase-catalyzed formation of H2O2) with detection limits (3σ) of 10 nM for H2O2 and 100 nM for glucose. The probe was employed for glucose determination in human plasma samples with satisfactory results.
Graphical abstract The effect of carbon nitride quantum dots (CN QDs) on Cu(II)-H2O2 chemiluminescence reaction was studied and the new CL system was applied for sensitive detection of glucose based on the glucose oxidase (GOx)-catalyzed formation of H2O2.
A voltammetric analytical assay for the selective quantification of vanillin is described. It is based on the use of a gold nanoparticle-modified screen-printed carbon electrode (SPCE) modified with graphene quantum dots (GQD) in a Nafion matrix. The GQD were synthesized by an acidic thermal method and characterized by UV-Vis, photoluminescence, and FTIR spectroscopy. The modified SPCE displays a strongly enhanced response to vanillin. Linear sweep voltammetry (LSV) and differential pulse voltammetry (DPV) were applied to optimize the methods. The analytical assay has linear responses in the 13 to 660 μM and 0.66 to 33 μM vanillin concentration ranges. The detection limits are 3.9 μM and 0.32 μM when using LSV and DPV, respectively. The analytical assay is selective and stable. It was applied to the determination of vanillin in several food samples with satisfactory results. Recoveries from spiked samples ranged between 92.1 and 113.0%.
Graphical abstract The selective and sensitive quantification of vanillin is carried out by the use of a gold nanoparticle-modified screen-printed carbon electrode modified with graphene quantum dots in a Nafion matrix.
A reagentless third generation electrochemical glucose biosensor was fabricated based on wiring the template enzyme glucose oxidase (GOx) with graphene nanoribbons (GN) in order to create direct electron transfer between the co-factor (flavin adenine dinucleotide, FAD) and the electrode. The strategy involved: (i) isolation of the apo-enzyme by separating it from its co-enzyme; (ii) preparation of graphene nanoribbons (GN) by oxidative unzipping of multi-walled carbon nanotubes; (iii) adsorptive immobilization of GNs on the surface of a screen printed carbon electrode (SPCE); (iv) covalent attachment of FAD to the nanoribbons; (v) recombination of the apo-enzyme with the covalently bound FAD to the holoenzyme; and (vi) stabilization of the bio-layer with a thin membrane of Nafion. The biosensor (referred to as GN/FAD/apo-GOx/Nafion/SPCE) is operated at a potential of +0.475 V vs Ag/AgCl/{3 M KCl} in flow-injection mode with an oxygen-free phosphate buffer (pH 7.5) acting as a carrier. The signals are linearly proportional to the concentration of glucose in the range from 50 to 2000 mg?L?1 with a detection limit of 20 mg?L?1. The repeatability (10 measurements, at 1000 mg?L?1 glucose) is ±1.4% and the reproducibility (5 sensors, 1000 mg?L?1 glucose) is ±1.8%. The biosensor was applied to the determination of glucose in human serum.
Graphical abstract Wiring of the apo-enzyme of glucose oxidase (apo-GOx) with graphene nanoribbons (GN) bound to FAD at a screen-printed carbon electrode (SPCE). Cyclic voltammetric and amperometric responses to various glucose concentrations.
A molecularly imprinted polymer (MIP) and a nanocomposite prepared from gold nanoparticles (AuNP) and poly(3,4-ethylenedioxythiophene)/poly(styrene sulfonate) (PEDOT:PSS) were deposited on a screen-printed carbon electrode (SPCE). The nanocomposite was prepared by one-pot simultaneous in-situ formation of AuNPs and PEDOT:PSS and was then inkjet-coated onto the SPCE. The MIP film was subsequently placed on the modified SPCE by co-electrodeposition of o-phenylenediamine and resorcinol in the presence of the antibiotic nitrofurantoin (NFT). Using differential pulse voltammetry (DPV), response at the potential of ~ 0.1 V (vs. Ag/AgCl) is linear in 1 nM to 1000 nM NFT concentration range, with a remarkably low detection limit (at S/N?=?3) of 0.1 nM. This is two orders of magnitude lower than that of the control MIP sensor without the nanocomposite interlayer, thus showing the beneficial effect of AuNP-PEDOT:PSS. The electrode is highly reproducible (relative standard deviation 3.1% for n?=?6) and selective over structurally related molecules. It can be re-used for at least ten times and was found to be stable for at least 45 days. It was successfully applied to the determination of NFT in (spiked) feed matrices and gave good recoveries.
Graphical abstract Schematic representation of a voltammetric sensor for the determination of nitrofurantoin. The sensor is based on a screen-printed carbon electrode (SPCE) modified with an inkjet-printed gold nanoparticles-poly(3,4-ethylenedioxythiophene):poly(styrene sulfonate) nanocomposite and a molecularly imprinted polymer.
A method is described for the synthesis of a nanocomposite containing FeOOH and N-doped carbon nanosheets. The nanocomposite was synthesized by a hydrothermal method using a Fe3O4/chitosan nanocomposite as the precursor. The nanocomposite displays peroxidase-like activity and catalyzes the oxidation of 3,3′,5,5′-tetramethylbenzidine (TMB) by H2O2. This results in the formation of a blue colored product with an absorption maximum at 652 nm in the UV-vis spectra. Based on these findings, colorimetric assays were worked out for both hydrogen peroxide and glucose. The H2O2 assay works in the 5 to 19 μM concentration range, and the limit of detection is 5 nM. The glucose assay works in the 8 μM to 0.8 mM concentration range and has a 0.2 μM detection limit. The method was successfully applied to the determination of glucose in human urine.
Graphical abstract Schematic of the hydrothermal synthesis of a FeOOH/N-doped carbon nanocomposite. It was used to replace peroxidase enzyme for the catalytic oxidation of 3,3′,5,5′-tetramethylbenzidine (TMB) in a visual colorimetric test for glucose in human urine.
Disposable screen-printed carbon arrays modified with gold nanoparticles (AuNPs) are described. The AuNP-modified screen-printed carbon arrays, designated as AuNP-SPCE arrays, were characterized by cyclic voltammetry and electrochemical impedance spectroscopy. The AuNP-SPCE arrays display excellent electrocatalytic activity towards lead and copper. Two well-defined and fully resolved anodic stripping peaks, at 20 mV for Pb(II) and at 370 mV for Cu(II), both vs. Ag/AgCl, can be seen. Square wave anodic stripping voltammetry was used to simultaneously analyze Pb(II) and Cu(II) in their binary mixtures in tap water. The linear working range for Pb(II) extends from 10 μg.L?1 to 100 μg.L?1 with a sensitivity of 5.94 μA.μg?1.L.cm?2. The respective data for Cu(II) are a working range from 10 μg.L?1 to 150 μg.L?1 with a sensitivity of 3.52 μA.μg?1.L.cm?2. The limits of detection (based on 3× the baseline noise) are 2.1 ng.L?1 and 1.4 ng.L?1, respectively. In our perception, this array is particularly attractive because Pb(II) and Cu(II) can be determined at rather low working potentials which makes the method fairly selective in that it is not significantly interfered by other electroactive species that require higher reduction potentials.
Graphical abstract Fabrication, characterization and electrochemical behavior of gold nanoparticles modified screen-printed carbon arrays towards lead and copper in tap water.
A composite consisting of chitosan containing azidomethylferrocene covalently immobilized on sheets of reduced graphene oxide was drop-casted on a polyester support to form a screen-printed working electrode that is shown to enable the determination of nitrite by cyclic voltammetry and chronoamperometry. Both reduction and oxidation of nitrite can be accomplished due to the high electron-transfer rate of this electrode. Under optimal experimental conditions (i.e. an applied potential of 0.7 V vs. Ag/AgCl in pH 7.0 solution), the calibration plot is linear in the 2.5 to 1450 μM concentration range, with an ~0.35 μM limit of detection (at a signal-to-noise ratio of 3). The sensor was successfully applied to the determination of nitrite in spiked mineral water samples, with recoveries ranging between 95 and 101 %.
Graphical abstract We describe the design of ferrocene-functionalized reduced graphene oxide electrode and its electrocatalytic properties towards the determination of nitrite. Compared to a reduced graphene oxide electrode, the sensor exhibits enhanced electrocatalytic activity towards both oxidation and reduction of nitrite.
Carbon nanotubes, graphenes, and their hybridized composites with nanoparticles have been attempted to establish a direct electrical communication between the recognition biomolecule and its underlying electrode surface. This review (with 133 refs.) focuses on advances, strategies and technical challenges in the development of reagentless electrochemical biosensors for glucose with enhanced detection sensitivity, selectivity, and simplicity. Specifically, the review commences with a discussion of the relevance of direct electron transfer (DET) in biosensing together with the fundamental of electro-enzymology and kinetics. General aspects of glucose oxidase (GOx), the most popular enzyme with a flavin cofactor, are discussed in view of its historical and important role in the development of electrical biosensors for blood glucose. The next section assesses DET of GOx based on the Marcus theory and the Laviron formalism. The reorganizational energy of the Marcus model and the overpotential play an important role in reaction kinetics and affect the rate of electron transfer significantly. The presence of nanomaterials, particularly for graphene oxide, decreases the electron transfer distance between the enzyme redox center and the underlying electrode surface well beyond 15 Å. The improper Marcus-Hush-Chidsey integral is now simplified to estimate the rate of electron transfer with very good accuracy. Critiques, technical challenges, and future possibilities of glucose electrodes with respect to DET are also presented and discussed.
Graphical abstract This review (with 133 refs.) focuses on advances, strategies and technical challenges in the development of reagentless electrochemical biosensors for glucose with enhanced detection sensitivity, selectivity, and simplicity.
We describe the electrochemical preparation of bismuth nanoribbons (Bi-NRs) with an average length of 100 ± 50 nm and a width of 10 ± 5 μm by a potentiostatic method. The process occurs on the surface of a glassy carbon electrode (GCE) in the presence of disodium ethylene diamine tetraacetate that acts as a scaffold for the growth of the Bi-NRs and also renders them more stable. The method was applied to the preparation of Bi-NRs incorporated into reduced graphene oxide. This nanocomposite was loaded with the enzyme glucose oxidase onto a glassy carbon electrode. The resulting biosensor displays an enhanced redox peak for the enzyme with a peak-to-peak separation of about 28 mV, revealing a fast electron transfer at the modified electrode. The loading of the GCE with electroactive GOx was calculated to be 8.54 × 10−10 mol∙cm−2, and the electron transfer rate constant is 4.40 s−1. Glucose can be determined (in the presence of oxygen) at a relatively working potential of −0.46 V (vs. Ag|AgCl) in the 0.5 to 6 mM concentration range, with a 104 μM lower detection limit. The sensor also displays appreciable repeatability, reproducibility and remarkable stability. It was successfully applied to the determination of glucose in human serum samples.
A potentiostatic method was used to prepare reduced graphene oxide and bismuth nanoribbons nanocomposite on a glassy carbon electrode. This nanocomposite was loaded with enzyme glucose oxidase to fabricate a glucose biosensor.
This article reviews the progress made in the past 5 years in the field of direct and non-enzymatic electrochemical sensing of glucose. Following a brief discussion of the merits and limitations of enzymatic glucose sensors, we discuss the history of unraveling the mechanism of direct oxidation of glucose and theories of non-enzymatic electrocatalysis. We then review non-enzymatic glucose electrodes based on the use of the metals platinum, gold, nickel, copper, of alloys and bimetals, of carbon materials (including graphene and graphene-based composites), and of metal-metal oxides and layered double hydroxides. This review contains more than 200 refs.
Figure This article reviews the history of unraveling the mechanism of direct electrochemical glucose oxidation and the attempts to successfully develop non-enzymatic electrochemical glucose sensors over the past 5 years.
Reduced graphene oxide (RGO) was used to construct a bienzyme biosensor containing horseradish peroxidase (HRP) and glucose oxidase (GOx). A poly(toluidine blue) (pTB) film containing RGO acted as both enzyme immobilization matrix and electron transfer mediator. The bienzyme biosensor was characterized by electrochemical techniques and displays a highly sensitive amperometric response to glucose and hydrogen peroxide (H2O2) at a potential as low as −0.1 V (vs. SCE). It is shown that use of RGO causes a strong enhancement on the amperometric responses. H2O2 formed by the action of GOx in the presence of oxygen can be further reduced by HRP in the pTB film contacting the RGO modified electrode. In the absence of oxygen, glucose oxidation proceeds by another mechanism in which electron transfer occurs from GOx to the electrode and with pTB acting as the mediator. Amperometric responses to glucose and H2O2 follow Michaelis-Menten kinetics. The experimental conditions were optimized, and under these conditions glucose can be determined in the 80 μM to 3.0 mM range with a detection limit of 50 μM. H2O2, in turn, can be quantified in up to 30.0 μM concentration with a detection limit of 0.2 μM. The bienzyme biosensor is reproducible, repeatable and stable. Finally, it has been successfully applied to the determination of glucose in plasma samples.
Schematic representation of glocuse detection at GCE/RGO/pTB-HRP-GOx.
Graphite-like carbon nitride ? Fe3O4 magnetic nanocomposites were synthesized by a chemical co-precipitation method. The nanocomposites were characterized by transmission electron microscopy, X-ray diffraction, FTIR spectroscopy, X-ray photoelectron spectroscopy and magnetization hysteresis loops. The nanocomposites exhibit enhanced peroxidase-like activity (compared to that of graphite-like carbon nitride or Fe3O4 NPs). More specifically, they are capable of catalyzing the oxidation of different peroxidase substrates (such as TMB, ABTS or OPD) by H2O2 to produce the typical color reactions (blue, green or orange). The nanocomposites retain their magnetic properties and can be separated by an external magnet. On the basis of these findings, a highly sensitive and selective method was applied to the determination of H2O2 and glucose (by using glucose oxidase). It was successfully applied to the determination of glucose in (spiked) human serum. Compared to other nanomaterial-based peroxidase mimetics, the one described here provides distinctly higher sensitivity for both H2O2 and glucose, with detection limits as low as 0.3 μM and 0.25 μM, respectively.
Graphical abstract The magnetic carbon nitride nanocomposite exhibits enhanced peroxidase-like activity that is much larger than that of graphite-like carbon nitride or Fe3O4 NPs alone. This finding was applied to design a highly sensitive and selective colorimetric assay for H2O2 and glucose.
We report on a sensitive and selective fluorescent assay utilizing native carbon dots (CDs) as signal transducers. The optical probes 2,2′-azinobis(3-ethylbenzothiazoline-6-sulfonate) (ABTS) or 3,3′-diaminobenzidine (DAB) were employed as substrates of horseradish peroxidase (HRP). It was found that the corresponding oxidation products (ox-ABTS or ox-DAB) quench the fluorescence of CDs, mainly via photoinduced electron transfer in case of ox-ABTS, and via aggregation and inner filter effect in case of ox-DAB. By coupling with bienzyme (glucose oxidase and HRP)-mediated biocatalytic reactions, the method was applied to the determination of hydrogen peroxide and glucose. In case of ABTS as the substrate of HRP, a wide linear range (0.05 to 100 μM) and a very low detection limit (10 nM) for glucose were attained. The method was applied to the determination of glucose in human serum and the results were found to agree well with data provided by a local hospital.
Graphical abstract In this work, a sensitive and selective fluorescent assay was developed for probing the enzymatic substrates of hydrogen peroxide and glucose which utilized native carbon dots (CDs) as signal transducer.
The authors describe an enzyme-free amperometric method for the determination of glucose at nanomolar levels at near neutral pH values. A hybrid nanostructure composed of molybdenum disulfide and copper sulfide (MoS2-CuS) was prepared using L-cysteine as both the sulfur donor and the reducing agent. The nanohybrid was then immobilized on a glassy carbon electrode (GCE) by incorporating it into a film of poly(vinyl butyral). Transmission electron microscopy and Raman spectroscopy were utilized to characterize the MoS2-CuS nanohybrids. Three modified GCEs (MoS2/GCE, CuS/GCE and MoS2-CuS/GCE) were investigated with respect to their sensitivity to glucose, and the MoS2-CuS/GCE was found to perform best in displaying a limit of detection as low as 0.3 μM in pH 7.2 buffer at an applied potential of +0.18 V (versus Ag/AgCl). The repeatability and intermediate precision are below 7.0% at 0.05, 0.5 and 1.0 mM concentration levels. The method was applied to the determination of glucose in spiked human serum samples, and recoveries were between 92.3 and 110.7%. This detection scheme is rapid and cost-effective. Natural enzymes and additional electron mediators are not required.
An electrochemical non-enzymatic glucose sensor based on copper nanorods (CuNRs) was developed. The CuNRs were characterized by scanning electron microscopy, transmission electron microscopy, X-ray diffraction spectroscopy, and X-ray photoelectron spectroscopy. The results display a layer of rough cuprous oxide that is formed on the surface of CuNRs. The CuNR- modified glassy carbon electrode exhibits an outstanding capability in terms of nonenzymatic sensing of glucose. The sensor displays high sensitivity (1490 μA?mM?1?cm?2), fast response time (less than 5 s), a low detection limit of 8 nM (S/N = 3), long term stability, and excellent anti-fouling ability. The sensor was applied to the detection of glucose in (spiked) human serum and in black ice tea, with relative standard deviations (for n = 6) of 1.7 % and 1.9 %, respectively.
Graphical abstract The surface of Cu nanorods was covered with cuprous oxide, which increased the surface area of the nanorods and provided more catalytic active sites for the electro-oxidation of glucose. Good linearity and selectivity were obtained in glucose sensing.
We describe a chemical exfoliation method for the preparation of MoS2 nanosheets. The nanosheets were incorporated into poly(3,4-ethylenedioxythiophene) (PEDOT) by electrodeposition on a glassy carbon electrode (GCE) to form a nanocomposite. The modified GCE is shown to enable simultaneous determination of ascorbic acid (AA), dopamine (DA) and uric acid (UA). Due to the synergistic effect of MoS2 and PEDOT, this electrode displays better properties in terms of electrocatalytic oxidation of AA, DA and UA than pure PEDOT, which is illustrated by cyclic voltammetry and differential pulse voltammetry (DPV). Under optimum conditions and at pH 7.4, the respective sensitivities and best working potentials are as follows: AA: 1.20 A?mM?1?m?2, 30 mV; DA: 36.40 A?mM?1?m?2, 210 mV; UA: 105.17 A?mM?1?m?2, 350 mV. The calculated detection limits for AA, DA and UA are 5.83 μM, 0.52 μM and 0.95 μM, respectively. The modified electrode was applied to the detection of the three species in human urine samples and gave satisfactory results.
Graphical abstract MoS2 nanosheets were prepared by a facile chemical exfoliation method. MoS2 and poly(3,4-ethylenedioxythiophene) nanocomposite modified glassy carbon electrodes were fabricated, which are shown to enable simultaneous determination of ascorbic acid, dopamine and uric acid with high sensitivity and selectivity.
