A label-free and single-step method is reported for rapid and highly sensitive detection of bisphenol A (BPA) in aqueous samples. It utilizes an aptamer acting as a probe molecule immobilized on a commercially available array of interdigitated aluminum microelectrodes. BPA was quantified by measuring the interfacial capacitance change rate caused by the specific binding between bisphenol A and the immobilized aptamer. The AC signal also induces an AC electrokinetic effect to generate microfluidic motion for enhanced binding. The capacitive aptasensor achieves a limit of detection as low as 10 fM(2.8 fg ⋅ mL − 1) with a 20 s response time. The method is inexpensive, highly sensitive, rapid and therefore provides a promising technology for on-site detection of BPA in food and water samples.
A. AC electrokinetics effect plays a vital role in BPA detection by introducing microfluidic movement to accelerate the molecular transport to the electrode surface.
B. The ACEK capacitive aptasensor has a limit of detection as low as 10 fM (2.8 fg ⋅ mL − 1) with a 20-s response time.
Alloy nanoparticles of the type PtxFe (where x is 1, 2 or 3) were synthesized by coreduction with sodium borohydride in the presence of carbon acting as a chemical support. The resulting nanocomposites were characterized by scanning electron microscopy and X-ray diffraction. The nanocomposite was placed on a glassy carbon electrode, and electrochemical measurements indicated an excellent catalytic activity for the oxidation of glucose even a near-neutral pH values and at a working voltage as low as 50 mV (vs. SCE). Under optimized conditions, the sensor responds to glucose in the 10.0 μM to 18.9 mM concentration range and with a 3.0 μM detection limit (at an S/N ratio of 3). Interferences by ascorbic acid, uric acid, fructose, acetamidophenol and chloride ions are negligible.
Nonenzymatic sensing of glucose is demonstrated at neutral pH values and low working potential using a glassy carbon electrode modified with platinum-iron alloy nanoparticles on a carbon support.
We describe the modification of a carbon paste electrode (CPE) with multiwalled carbon nanotubes (MWCNT) and an ionic liquid (IL). Electrochemical studies revealed an optimized composition of 60 % graphite, 20 % paraffin, 10 % MWCNT and 10 % IL. In a next step, the optimized CPE was modified with palladium nanoparticles (Pd-NPs) by applying a double-pulse electrochemical technique. The resulting electrode was characterized by scanning electron microscopy, energy dispersive X-ray spectroscopy, X-ray diffraction, cyclic voltammetry, and electrochemical impedance spectroscopy. It gives three sharp and well separated oxidation peaks for ascorbic acid (AA), dopamine (DA), and uric acid (UA), with peak separations of 180 and 200 mV for AA-DA and DA-UA, respectively. The sensor enables simultaneous determination of AA, DA and UA with linear responses from 0.6 to 112, 0.1 to 151, and 0.5 to 225 μM, respectively, and with 200, 30 and 150 nM detection limits (at an S/N of 3). The method was successfully applied to the determination of AA, DA, and UA in spiked samples of human serum and urine.
The CPE was modified with multiwalled carbon nanotubes and an ionic liquid. After optimization the electrode was further modified with palladium nanoparticles. The resulting electrode gives three sharp and well separated oxidation peaks for ascorbic acid, dopamine and uric acid
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
We describe an electrochemical sensor for nitric oxide that was obtained by modifying the surface of a nanofiber carbon paste microelectrode with a film composed of hexadecyl trimethylammonium bromide and nafion. The modified microelectrode displays excellent catalytic activity in the electrochemical oxidation of nitric oxide. The mechanism was studied by scanning electron microscopy and cyclic voltammetry. Under optimal conditions, the oxidation peak current at a working voltage of 0.75 V (vs. SCE) is related to the concentration of nitric oxide in the 2 nM to 0.2 mM range, and the detection limit is as low as 2 nM (at an S/N ratio of 3). The sensor was successfully applied to the determination of nitric oxide released from mouse hepatocytes.
NO electrochemical sensor based on CTAB-Nafion/CNFPME was fabricated through a simple method and applied to detect NO released from mouse hepatocytes successfully.
Thin-layered molybdenum disulfide (MoS2) was intercalated, via ultrasonic exfoliation, into self-doped polyaniline (SPAN). This material, when placed on a glassy carbon electrode (GCE), exhibits excellent electrical conductivity and synergistic catalytic activity with respect to the detection of bisphenol A (BPA). The electrochemical response of the modified GCE to BPA was investigated by cyclic voltammetry and differential pulse voltammetry. Under optimal conditions, the oxidation peak current (measured best at 446 mV vs. SCE) is related to the concentration of BPA in the range from 1.0 nM to 1.0 μM, and the detection limit is 0.6 nM.
Thin-layered molybdenum disulfide (MoS2) was intercalated into self-doped polyaniline (SPAN) via ultrasonic exfoliation. The special conjugated structure and functional groups of MoS2-SPAN composite help to adsorb BPA easily. MoS2-SPAN has a synergistic effect for catalyzing the oxidation of BPA. The BPA electrochemical sensor based on MoS2-SPAN has a high sensitivity and low detection limit.
We describe a nanostructured immunosensor for the cardiovascular biomarker netrin 1. A glassy carbon electrode was consecutively modified with multi-walled carbon nanotubes (MWCNTs), nafion (to retain the MWCNTs), thionine-coated gold nanoparticles (Thi@AuNPs), and monoclonal antibodies against netrin 1. The modified electrode was characterized by transmission electron microscopy, cyclic voltammetry, differential pulse voltammetry, UV-visible spectrophotometry and X-ray diffraction. The presence of Thi@AuNPs warrants direct and convenient immobilization of the antibody. This immunoelectrode enables netrin 1 to be determined, best at a voltage of −300 mV (vs. SCE), with a limit of detection of 30 fg mL−1 (at an S/N ratio of 3) after a 50 min incubation time. The detection range extends from 0.09 to 1800 pg∙mL−1. The method is simple, sensitive, specific and reproducible. We presume this stable and reproducible biosensor to be useful for the early detection of cardiovascular diseases.
A high sensitivity immunoassay was developed for the detection of netrin 1 based on multi-walled carbon nanotubes, thionine and gold nanoparticles. Its excellent performance is ascribed to the good conductivity of MWCNTs and the combination of materials.
We describe an electrochemical bioassay for the detection of the activity of methyltransferase (MTase), and for screening this enzyme’s inhibitors. The assay is based on the conjugation of a hemin to a G-quadruplex that enables enzymatic signal amplification with the aid of exonuclease III (ExoIII). In the first step, double-stranded DNA containing the quadruplex-forming oligomer is assembled on the surface of a gold electrode and then methylated by DNA adenine methyltransferase (DAM). After cleaved by endonuclease DpnI, the methylated DNA is digested by ExoIII and the quadruplex-forming oligomers are liberated. This leads to the formation of a hemin/G-quadruplex (in presence of hemin and of potassium ions). The hemin/G-quadruplex catalyzes the oxidization of hydroquinone by H2O2 and the benzoquinone was formed to generate electrochemical signal. Finally, the gold electrode modified with reduced graphene oxide was used as working electrode for performing differential pulse voltammetry. The method has a detection limit of 0.31 unit · mL−1. A study on the inhibition of MTase showed it was inhibited by epicatechin with an IC50 value of 157 μM.
We describe an electrochemical bioassay for the detection of the activity of methyltransferase and for screening for its inhibitors. Due to the conjugation of a hemin to a G-quadruplex, strong enzymatic signal amplification is enabled with the aid of exonuclease III.
We describe a simple and homogenous fluorimetric method for sensitive determination of DNA. It is based on target-triggered isothermal cycling and a cascade exponential amplification reaction that generates a large amount of a G-quadruplex. This results in strong fluorescence signal when using thioflavin T as a G-quadruplex-specific light-up fluorescent probe. Tedious handling after amplification is widely eliminated by the addition of thioflavin T. No other exogenous reagent is required. This detection platform is inexpensive and rapid, and displays high sensitivity for target DNA, with a detection limit as low as 91 pM.
The addition of target DNA can trigger the isothermal exponential amplification reaction to generate a large amount of G-quadruplex sequence oligonucleotides and then employ thioflavin T (Th T) (a G-quadruplex-specific light-up dye) as signal output for sensitive DNA detection.
This article describes an electrochemical sensor for the dye additive Sunset Yellow (SY). It consists of a carbon paste electrode modified with nanostructured resorcinol-formaldehyde (RF) resin. The RF resin warrants strong signal enhancement and a strongly increased oxidation peak currents of SY at 0.66 V (vs. SCE). The effects of pH value, amount of RF polymer, accumulation potential and time were optimized. The sensor has a linear response to SY in the 0.3 to 125 nM concentration range, and the limit of detection is 0.09 nM after a 2-min accumulation time. The electrode was applied to the analysis of samples of wastewater and drinks, and the results are consistent with those obtained by HPLC.
Nanostructured resorcinol-formaldehyde (RF) resin was prepared and used as a material for electrochemical determination of Sunset Yellow.
We report on a sensitive aptamer-antibody interaction-based assay for cytochrome c (Cyt c) using electrochemical impedance. 4-Amino benzoic acid is used for the oriented immobilization of aminated aptamers onto multi-walled carbon nanotubes on the surface of a screen-printed electrode via electrochemical grafting. Impedance was measured in a solution containing the redox system ferro/ferricyanide. The change in interfacial charge transfer resistance (Rct) experienced by the redox marker was recorded to confirm the formation of a complex between aptamer and the target (Cyt c). A biotinylated antibody against cytochrome c was then used in a sandwich type of assay. The addition of streptavidin conjugated to gold nanoparticles and signal enhancement by treatment with silver led to a further increase in Rct. Under optimized conditions, a detection limit as low as 12 pM was obtained. Cross-reactivity against other serum proteins including fibrinogen, BSA and immunoglobulin G demonstrated improved selectivity.
Sensitive and selective assay for cytochrome c protein using aptamer linked to multi-walled carbon nanotube screen printed electrode via diazonium electrochemical grafting and specific biotinylated antibody to improve selectivity. Detection can be based on electrochemical impedance spectroscopy, or using a streptavidin-gold nanoparticle conjugate.
We describe a novel procedure for the synthesis of nitrogen-doped reduced graphene oxide (N-rGO). It is based on the thermal reduction of GO (dispersed in water) with sodium diethyldithiocarbamate that acts as both the reducing agent and the source for nitrogen. The surface morphology of the N-rGO is characterized using high resolution transmission electron microscopy. X-ray photoelectron spectroscopy was carried out to study the composition of their surface, and Raman spectroscopy was performed to study the level of doping with nitrogen and the structural order. The N-rGO was deposited on a glassy carbon electrode (GCE), and the resulting electrode utilized as a sensing platform for 4-nitrophenol (4-NP). The modified GCE exhibits a well-defined oxidation peak current that is about ten times larger when compared to that of a bare GCE. The electron transfer number, proton transfer number and electron transfer rate constant (ks 1.046 s−1) were determined. At optimized conditions, the oxidation peak current is linearly related to the concentration of 4-NP in the 20–500 nM range, with a correlation coefficient of 0.9917. The detection limit (at an SNR of 3) is 7 nM. The method was successfully applied to the analysis of waters spiked with 4-NP. Recoveries range from 97.8 to 102.6 %, and no interferences are found for common inorganic cations and anions.
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This study introduces a new surface-renewable electrode based on a sol–gel derived graphene ceramic composite. The electrode was prepared by dispersing graphene nanosheets into a solution of the sol–gel precursors containing methyl triethoxysilane in methanol and hydrochloric acid. During hydrolysis of methyl triethoxysilane, the graphene nanosheets are trapped in the gel. After moulding and drying the composite, it can be used as a surface-renewable electrode to which we refer as a graphene ceramic composite electrode (GCCE). Cyclic voltammograms of the hexacyanoferrate(II/III) model redox system at the GCCE were compared to those obtained with a conventional carbon ceramic electrode and showed a highly improved electron transfer rate at the GCCE. The electrocatalytic oxidation of ascorbic acid as a model analyte was then studied at working potential of 50 mV and over the 3–84 μM concentration range. It revealed a sensitivity of 6.06 μA μM−1 cm−2 and a detection limit of 0.82 μM. The GCCE was successfully applied to the determination of ascorbic acid in orange juice and urine samples. Advantages such as good mechanical and chemical stability, ease of fabrication, and reproducible preparation make the GCCE a potentially useful and widely applicable renewable electrode for use in routine analysis.
(Left) FESEM image and photograph of the graphene ceramic composite electrode (GCCE); (right) the cyclic voltammogram of the renewable GCCE in 5 mM K3[Fe(CN)6] solution containing 0.1 M KNO3 at scan rate of 100 mV s−1
A nanocomposite consisting of reduced graphene oxide decorated with palladium-copper oxide nanoparticles (Pd-CuO/rGO) was synthesized by single-step chemical reduction. The morphology and crystal structure of the nanocomposite were characterized by field-emission scanning electron microscopy, high resolution transmission electron microscopy and X-ray diffraction analysis. A 3-electrode system was fabricated by screen printing technology and the Pd-CuO/rGO nanocomposite was dropcast on the carbon working electrode. The catalytic activity towards glucose in 0.2 M NaOH solutions was analyzed by linear sweep voltammetry and amperometry. The steady state current obtained at a constant potential of +0.6 V (vs. Ag/AgCl) showed the modified electrode to possess a wide analytical range (6 μM to 22 mM), a rather low limit of detection (30 nM), excellent sensitivity (3355 μA∙mM−1∙cm−2) and good selectivity over commonly interfering species and other sugars including fructose, sucrose and lactose. The sensor was successfully employed to the determination of glucose in blood serum.
A highly sensitive nonenzymatic electrochemical sensor was fabricated using a Pd-CuO composite with reduced graphene oxide. The sensor has a wide detection range and was used to sense glucose in blood serum
A jelly-like form of carbon dots (C-dots) was prepared by microwave-assisted synthesis from citric acid in the presence of tetraoctylammonium bromide. The effect of the concentration of tetraoctylammonium bromide was examined. The synthesized carbon dots were characterized by UV–vis, XRD, FTIR, fluorescence and HR-TEM. Fluorescence extends from 350 to 600 nm, and the corresponding excitation wavelengths range from 300 to 460 nm. Quantum yields are at around 0.11. A cytotoxicity study showed carbon dots to be cell permeable and biocompatible which renders them appropriate for imaging applications. The dots were used to image HeLa cell lines via the blue fluorescence of the dots.
C-dots were synthesized from citric acid by microwave heating in presence of varying concentrations of tetraoctylammonium bromide (TOAB) as a micellar template. The excellent optical properties of the nanoparticles make them well suitable for bio-imaging of HeLa cells.
We report on an effective strategy for the enhancement in the sensitivity of localized surface plasmon resonance (LSPR). It is based on the use of gold-silver core-shell nanorods (Au-Ag-cs-NRs) immobilized on a glass substrate. The nanorods arrange themselves by self-assembly, and the resulting LSPR band of the Au-Ag-cs-NRs becomes sharper and more intense. The sensitivity to refractive index (RI) of the Au-Ag-cs-NRs on the glass support is ~281 nm per RI unit, which is better by about 30 % compared to gold nanorods immobilized on glass substrate. The system was applied to study the streptavidin-biotin affinity system which is widely used in biosciences. It is found that the red-shift of the LSPR peak linearly increases with the concentration of streptavidin in the 95 pM to 1.7 μM concentration range. The detection limit (at an S/N ratio of 3) is at 35 pM. The results reveal the merits of this approach in terms of label-free optical affinity sensing.
Au-Ag core-shell nanorods self-assembled on glass substrates. The refractive index sensitivity was enhanced obviously. A strategy to amplify the response and fabricate a label-free optical biosensor
We describe an electrochemical sensor for melamine based on a glassy carbon electrode (GCE) modified with reduced graphene oxide that was decorated with gold nanoparticles (AuNP/rGO). The AuNPs/rGO nanocomposite was synthesized by co-reduction of Au(III) and graphene oxide and characterized by transmission electron microscopy, Raman spectroscopy, X-ray diffraction and X-ray photoelectron spectroscopy. The response of the modified GCE to melamine was investigated by using hexacyanoferrate as an electrochemical reporter. It is found that the electrochemical response to hexacyanoferrate is increasingly suppressed by increasing concentration of melamine. This is attributed to competitive adsorption of melamine at the AuNP/rGO composite through the interaction between the amino groups of melamine and the AuNPs. The presence of rGO, in turn, provides a platform for a more uniform distribution of the AuNPs and enhances the electron transfer rate of the redox reaction. The findings were used to develop a sensitive method for the determination of melamine. Under optimized conditions, the redox peak current of hexacyanoferrate at a working voltage of 171 mV (vs. SCE) is linearly related to the concentration of melamine in 5.0 to 50 nM range. The method was successfully applied to the determination of melamine in food contact materials.
A simple electrochemical sensor based on gold nanoparticles decorated reduced graphene oxide was developed for highly sensitive measurement of melamine in food contact materials.
We have prepared molecularly imprinted beads with molecular recognition capability for target molecules containing the penicillanic acid substructure. They were prepared by (a) grafting mesoporous silica beads with 6-aminopenicillanic acid as the mimic template, (b) filling the pores with a polymerized mixture of methacrylic acid and trimethylolpropane trimethacrylate, and (c) removing the silica support with ammonium fluoride. The resulting imprinted beads showed good molecular recognition capability for various penicillanic species, while antibiotics such as cephalosporins or chloramphenicol were poorly recognized. The imprinted beads were used to extract penicillin V, nafcillin, oxacillin, cloxacillin and dicloxacillin from skimmed and deproteinized milk in the concentration range of 5–100 μg·L−1. The extracts were then analyzed by micellar electrokinetic chromatography by applying reverse polarity staking as an in-capillary preconcentration step, and this resulted in a fast and affordable method within the MRL levels, characterized by minimal pretreatment steps and recoveries of 64–90 %.
Penicillanic acid-imprinted beads prepared in preformed porous silica by an imprinting &; etching approach show selectivity towards β-lactams antibiotics. Molecularly imprinted solid phase extraction/micellar electrokinetic chromatography coupled with in-capillary preconcentration resulted in a fast and affordable method for penicillins in milk at MRL levels.
We report on an electrochemical method for the determination of the activity of trypsin. A multi-functional substrate peptide (HHHAKSSATGGC-HS) is designed and immobilized on a gold electrode. The three His residues in the N-terminal are able to recruit thionine-loaded graphene oxide (GO/thionine), a nanocover adopted for signal amplification. Once the peptide is cleaved under enzymatic catalysis by trypsin (cleavage site: Lys residue), the His residues leave the electrode, and the GO/thionine cannot cover the peptide-modified electrode anymore. Thus, the changes of the electrochemical signal of thionine, typically acquired at a voltage of -0.35 V, can be used to determine the activity of trypsin. A detection range of 1 × 10−4 to 1 U, with a detection limit of 3.3 × 10−5 U, can be achieved, which is better than some currently available methods. In addition, the method is highly specific, facile, and has the potential for the detection of trypsin-like proteases.
Graphene oxide was adopted as a nanocover for the development of a sensitive electrochemical method to detect the activity of trypsin.
We describe a new kind of electrochemical immunoassay for the peptide hormone prolactin. A glassy carbon electrode (GCE) was modified with a hybrid material consisting of graphene, single walled carbon nanotubes and gold nanoparticles (AuNPs) in a chitosan (CS) matrix. The graphene and the single wall carbon nanotubes were first placed on the GCE, and the AuNPs were then electrodeposited on the surface by cyclic voltammetry. This structure results in a comparably large surface for immobilization of the capturing antibody (Ab1). The modified electrode was used in a standard sandwich-type of immunoassay. The secondary antibody (Ab2) consisted of AuNPs with immobilized Ab2 and modified with biotinylated DNA as signal tags. Finally, alkaline phosphatase was bound to the biotinylated DNA-AuNPs-Ab2 conjugate via streptavidin chemistry. The enzyme catalyzes the hydrolysis of the α-naphthyl phosphate to form α-naphthol which is highly electroactive at an operating voltage as low as 180 mV (vs. Ag/AgCl). The resulting immunoassay exhibits high sensitivity, wide linear range (50 to 3200 pg∙mL‾1), low detection limit (47 pg∙mL‾1), acceptable selectivity and reproducibility. The assay provides a pragmatic platform for signal amplification and has a great potential for the sensitive determination of antigens other than prolactine.
The immunoassay for prolactin is based on a glassy carbon electrode modified with SWCNTs, graphene and antibody-coated gold nanoparticles, and a secondary antibody conjugated to other gold nanoparticles via a biotinylated DNA linker