Near infrared (NIR) emitting semiconductor quantum dots can be excellent fluorescent nanoprobes, but the poor biodegradability and potential toxicity limits their application. The authors describe a fluorescent system composed of graphene quantum dots (GQDs) as NIR emitters, and novel MnO2 nanoflowers as the fluorescence quenchers. The system is shown to be an activatable and biodegradable fluorescent nanoprobe for the “turn-on” detection of intracellular glutathione (GSH). The MnO2-GQDs nanoprobe is obtained by adsorbing GQDs onto the surface of MnO2 nanoflowers through electrostatic interaction. This results in the quenching of the NIR fluorescence of the GQDs. In the presence of GSH, the MnO2-GQDs nanoprobe is degraded and releases Mn2+ and free GQDs, respectively. This gives rise to increased fluorescence. The nanoprobe displays high sensitivity to GSH and with a 2.8 μM detection limit. It integrates the advantages of NIR fluorescence and biodegradability, selectivity, biocompatibility and membrane permeability. All this makes it a promising fluorescent nanoprobe for GSH and for cellular imaging of GSH as shown here for the case of MCF-7 cancer cells.
Graphical abstract A biodegradable NIR fluorescence nanoprobe (MnO2-GQDs) for the “turn-on” detection of GSH in living cell was established, with the NIR GQD as the fluorescence reporter and the MnO2 nanoflower as the fluorescence quencher.
The authors describe a rapid and sensitive method for the determination of the activity of scavenging hydrogen peroxide in which glucose oxidase–stabilized gold nanoclusters (AuNCs) were employed as a fluorescent nanoprobe. The AuNCs are synthesized by a biomineralization process and display an intense blue fluorescence peaking at 450 nm and a quantum yield of 1.1% under 360–nm excitation. The Fenton reaction induces quenching of fluorescence, and this effect can be used to determine H2O2 in the 0.5 to 10 μmol?L?1 concentration range. The substances displaying H2O2 scavenging activity prevent quenching and thus restore fluorescence. The intensity of restored fluorescence is directly related to the H2O2 scavenging activity of the antioxidant. The method was applied to the determination of the H2O2 scavenging activity of the model antioxidants ascorbic acid and tartaric acid which gave IC50 values of 7.4 and 19.1 μmol?L?1, respectively.
Graphical abstract Blue-emitting gold nanoclusters (AuNCs) were prepared by using GOx as both the reducing and stabilizing agents. The Fenton reaction induces quenching of fluorescence of the AuNCs, and is employed for fluorometric measurement of the H2O2 scavenging activity of the model antioxidants ascorbic acid and tartaric acid.
A multiplexed graphene oxide (GO) fluorescent nanoprobe is described for quantification and imaging of messenger RNAs (mRNAs) in living cells. The recognizing oligonucleotides (with sequences complementary to those of target mRNAs) were labeled with different fluorescent dyes. If adsorbed on GO, the fluorescence of the recognizing oligonucleotides is quenched. After having penetrated living cells, the oligonucleotides bind to target mRNAs and dissociate from GO. This leads to the recovery of fluorescence. Using different fluorescent dyes, various intracellular mRNAs can be simultaneously imaged and quantified by a high content analysis within a short period of time. Actin mRNA acts as the internal control. This GO-based nanoprobe allows mRNA mimics to be determined within an analytical range from 1 to 400 nM and a detection limit as low as 0.26 nM. Up to 3 intracellular mRNAs (C-myc, TK1, and actin) can be detected simultaneously in a single living cell. Hence, this nanoprobe enables specific distinction of intracellular mRNA expression levels in cancerous and normal cells. It can be potentially applied as a tool for detection of cancer progression and diagnosis.
Graphical abstract A multiplexed graphene oxide (GO)-based fluorescent nanoprobe is described for quantification and imaging of intracellular messenger RNAs. After penetrating living cells, the recovered fluorescence of the dissociated recognizing oligonucleotides can be analyzed , and this allows for simultaneous detection of up to 3 intracellular messenger RNAs.
The paper describes a fluorescent method for determination of Au(III) using molybdenum disulfide quantum dots (MoS2 QDs) that were prepared by a hydrothermal route using glutathione as a reductant. The photoluminescence of MoS2 QDs peaks at 416 nm if excited at 340 nm and is temporally stable even in presence of NaCl or when stored in the refrigerator for one year. Its quantum yield is 12.7 %. The blue-green fluorescence of MoS2 QDs is fairly specifically quenched by Au(III) ions and therefore presents a useful nanoprobe for this ion. Fluorescence intensity drops linearly with the concentration of Au(III) in the range from 0.5 to 1000 μM, and the lower detection limit is 64 nM. The quenching mechanism was investigated and it is concluded that the process is due to the reduction of Au(III) and the deposition of Au(0) on the surface of the MoS2 QDs. The nanoprobe was successfully applied to the determination of Au(III) in (spiked) environmental samples. A test stripe for Au(III) was obtained by soaking a piece of paper with a colloidal solution of the MoS2 QDs, and it was found that this stripe, after drying, can also be used to quantify Au(III) via fluorescence.
Graphical abstract Molybdenum disulfide quantum dots (MoS2 QDs) have a high quantum yield and show good stability. MoS2 QDs are shown to be a sensitive fluorescent probe for the determination of Au3+ ions in solution and with a test stripe via fluorescence quenching.
A sandwich-type electrochemical DNA sensor is described for the detection of oligonucleotides typical for MECP2 gene mutations. Palladium nanoparticles (PdNPs) and platinum nanoparticles (PtNPs) were used to synthesize flower-like PdPt nanodendrites (NDs) by a one-pot method. The PdPt NDs possess a high specific surface area and excellent catalytic capabilities. They served as the carrier for the signal DNA probe (SP) and simultaneously catalyze the reduction of hydrogen peroxide (H2O2). The PdPt NDs were modified with melamine, and this results in the formation of a PdPt-melamine network through stable interactions between the PdPt NDs and the three amino groups of each melamine molecule. The network exhibits excellent catalytic ability in enhancing the current signal response in the voltammetric detection of MECP2 gene mutation, best measured at ?0.4 V vs. SCE and using H2O2 as the electrochemical probe. In addition, gold nanoflowers were electrodeposited on the electrode interface in order to accelerate electron transfer and to capture the capture probe. The sensor is stable and can detect MECP2 gene mutations in the 1 fmol·L?1 to 1 nmol·L?1 concentration range, with a 0.33 fmol·L?1 lower detection limit at an S/N ratio of 3.
Graphical abstract Schematic presentation of electrodes for the determination of the X-linked gene methyl-CpG-binding protein 2 (MECP2). The sensor is based on the electrooxidation of added H2O2 by using the melamine modified palladium platinum bimetal nanodendrites as network signal amplification strategy. This versatile platform expands studies on the detection of monogenic disease.
We report on a non-enzymatic hydrogen peroxide (H2O2) sensor which makes use of a nanocomposite consisting of platinum nanoparticles (PtNPs) and chitosan-encapsulated graphite (graphite-CS). The composite was prepared by sonication of pristine graphite in chitosan (CS) in 5 % acetic acid. The PtNP decorated graphite-CS (graphite-CS/PtNPs) composite was prepared by electrodeposition of PtNPs on the graphite-CS modified glassy carbon electrode. The graphite-CS/PtNP composite was characterized by scanning electron microscopy, elemental analysis and FTIR spectroscopy. The modified electrode displays an enhanced reduction peak current for H2O2 when compared with electrodes modified with graphite/PtNPs and PtNPs. The modified electrode exhibits excellent electrocatalytic activity towards the reduction of H2O2, and the amperometric response is linear over the concentration range from 0.25 to 2890 μM. The sensitivity and the detection limit are 0.465 μA?μM ̄1 ? cm ̄2 and 66 nM, respectively. The sensor shows fast response (3 s) in detecting H2O2. It is also highly selective in the presence of potentially interfering compounds, and may therefore be used as a feasible platform for sensing H2O2 in real samples.
The authors describe a sensitive surface-enhanced Raman scattering (SERS)-based aptasensor for the detection of the food pathogen Vibrio parahaemolyticus. Nanostructures consisting of Fe3O4@Au particles wrapped with graphene oxide (GO) were used both as SERS substrates and separation tools. A first aptamer (apt 1) was immobilized on the Fe3O4@Au/GO nanostructures to act as a capture probe via the affinity binding of aptamer and V. parahaemolyticus. A second aptamer (apt-2) was modified with the Raman reporter molecule TAMRA to act as a SERS sensing probes that binds to the target the same way as the Fe3O4@Au/GO-apt 1. The sandwich formed between Fe3O4@Au/GO-apt 1/V. parahaemolyticus and apt 2-TAMRA can be separated with the aid of a magnet. The concentration of V. parahaemolyticus can be quantified by measurement of the SERS intensity of TAMRA. Under optimal conditions, the signal is linearly related to the V. parahaemolyticus concentration in the range between 1.4 × 102 to 1.4 × 106 cfu·mL?1, with a detection limit of 14 cfu·mL?1. Recoveries ranging from 98.5% to 105% are found when analyzing spiked salmon samples. In our perception, the assay described here is a useful tool for quantitation of V. parahaemolyticus in real samples.
Graphical abstract GO wrapped Fe3O4@Au nanostructures were synthesized as the substrate and modified with with a first aptamer (apt 1) to capture V. parahaemolyticus. TAMRA labelled aptamer 2 was then used as signal probe. The V. parahaemolyticus concentrations are closely related to the Raman intensity of TAMRA.
The authors describe a fluorescent probe for sensitive and selective determination of quercetin, an indicator for the freshness of drinks. The probe consists of silica ball encapsulated graphitic carbon nitride (g-C3N4) modified with a molecularly imprinted polymer (MIP). It was synthesized via reverse microemulsion. The resulting MIP@g-C3N4 nanocomposite was characterized by fluorescence spectroscopy, transmission electron microscopy, Fourier transform infrared spectroscopy, and X-ray powder diffraction. Quercetin quenches the fluorescence of the MIP@g-C3N4 probe. The effect was used to quantify quercetin in grape juice, tea juice, black tea, and red wine by fluorometry (λexc?=?350 nm, λem?=?460 nm). Response is linear in the 10–1000 ng mL?1 quercetin concentration range. The detection limit is 2.5 ng mL?1, recoveries range between 90.7 and 94.1%, and relative standard deviations are between 2.1 and 5.5%.
Graphical abstract Schematic of the synthesis of the MIP@g-C3N4 by a reverse microemulsion method. The probe was applied for the selective recognition and fluorometric determination of quercetin.
The authors describe a highly efficient photoelectrochemical (PEC) scheme for the determination of hydrogen peroxide (H2O2). BiVO4 microrods were hydrothermally synthesized and deposited on fluorine - doped tin oxide (FTO) glass which acts as the working electrode. Scanning electron microscopy, X-ray powder diffraction and Raman spectroscopy were utilized for the characterization of the microrods. On irradiation with visible light, the holes generated in the microrods are capturing electrons from H2O2 to produce a photocurrent at an operating potential of 0 V vs. Ag/AgCl. Under optimal conditions, the photocurrent increases with the concentration of H2O2 in the range from 50 μmol·L?1 to 1.5 mmol·L?1, and the limit of detection is 8.5 μmol·L?1 (at 3σ). A repeatability and intermediate precision of ≤6.6% was accomplished at H2O2 levels of 0.1, 0.5 and 1.0 mmol·L?1. The method was applied to the determination of H2O2 in spiked sterilized milk samples and gave satisfactory results. As the method works at zero potential, the photocurrent can be measured with simple instrumentation such as digital multimeters, and this will enable expensive electrochemical workstations to be replaced in future.
Graphical abstract An enzyme-free photoelectrochemical sensing strategy is described for sensitive determination of hydrogen peroxide in foodstuff using fluorine-doped tin oxide electrode modified with BiVO4 microrods.
A highly selective electrochemical sensor was fabricated based on a modified carbon paste electrode with zinc ferrite nanoparticles (ZnFe2O4 NPs). The nanocomposite has attractive properties such as high surface-to-volume ratio and good electrocatalytic activity towards the drugs acetaminophen (AC), epinephrine (EP), and melatonin (MT), best at working voltages of 0.35, 0.09 and 0.55 V (vs. Ag/AgCl), respectively. The linear ranges (and detection limits) are 6.5–135 (0.4) μmol L?1 for AC, 5–100 (0.7) μmol L?1 for EP, and 6.5–145 (3) μmol L?1 for MT.
Graphical abstract A novel electrochemical sensor based on a modified carbon paste electrode with zinc ferrite nanoparticles (ZnFe2O4) for the simultaneous detection of the acetaminophen, epinephrine and melatonin was fabricated
A multifunctional fluorescent probe is synthesized for the determination of adenosine 5′-triphosphate (ATP). The 6-carboxyfluorescein-labeled aptamer (FAM-aptamer) was bound to the surface of magnetite nanoparticles coated with polydopamine (Fe3O4@PDA) by π-π stacking interaction to form the multifunctional probe. The probe has three functions including recognition, magnetic separation, and yielding a fluorescent signal. In the presence of ATP, FAM-aptamer on the surface of the probe binds to ATP and returns to the solution. Thus, the fluorescence of the supernatant is enhanced and can be related to the concentration of ATP. Fluorescence intensities were measured at excitation/emission wavelengths of 494/526 nm. Response is linear in the 0.1–100 μM ATP concentration range, and the detection limit is 89 nM. The probe was applied to the quantitation of ATP in spiked human urine and serum samples, with recoveries ranging between 94.8 and 102%.
Graphical abstract A multifunctional fluorescent probe based on the use of FAM-aptamer and Fe3O4@PDA is described for the determination of ATP in spiked human urine and serum samples. FAM-aptamer: 6-carboxyfluorescein-labeled aptamer; Fe3O4@PDA: magnetite nanoparticles coated with polydopamine. ATP: adenosine 5′-triphosphate.
A dual enhancing strategy has been employed to develop a sandwich type of electrochemical immunoassay for the prostate specific antigen (PSA). The signal is enhanced by using Pt-Cu hierarchical trigonal bipyramid nanoframes (HTBNFs) and a composite consisting of Fe3O4 nanoparticles and reduced graphene oxide in polydopamine that serve to capture the primary antibody (Ab1). This nanocomposite shows better electrical conductivity than Fe3O4 and reduced graphene oxide (RGO), respectively, alone. The Pt-Cu HTBNFs were used to label the secondary antibody (Ab2) and act as tags for signal amplification by virtue of their outstanding electrochemical reduction activity towards H2O2. At a working potential of +0.1 V (vs. SCE), the interference by dissolved oxygen can be avoided. This immunoassay is highly sensitive, with a linear range that extends from 0.1 pg?mL?1 to 5 ng?mL?1 and an ultralow detection limit of 0.03 pg?mL?1.
Graphical abstract Schematic of the dual amplification strategy in the immunosensor for the prostate specific antigen (PSA) that is based on the use of a first antibody (Ab1) conjugated to a Fe3O4-reduced graphene oxide nanocomposite (Fe3O4-RGO), and of Pt-Cu trigonal bipyramid nanoframes as a label for the second antibody (Ab2).
This study describes an amperometric sensor for hydrogen peroxide (H2O2) that uses an ITO glass electrode which was modified with a nanocomposite consisting of electrochemically reduced graphene oxide and gold nanoclusters (AuNCs). The sensor was used to quantify extracellular H2O2 released from human neuroblastoma cells of type SH-SY5Y. The calibration plot, established best at a working voltage of ?0.4 V (vs. Ag/AgCl) is linear in the 40 nmol?L?1 to 2 μmol?L?1 concentration range, and the detection limit is 20 nmol?L?1 (at a signal-to-noise ratio of 3). The method was further applied to study bupivacaine-induced cell damage and the protective effects of α-lipoic acid. The study indicated that pretreatment of the cells with lipoic acid retards cell damage induced by bupivacaine. The sensor can be easily fabricated, is disposable and highly sensitive. The sensor is perceived to represent an alternative for studying the interactions of drugs with cells, and as an effective tool to quantify cell-secreted H2O2.
Graphical abstract One-step electrochemical synthesis of graphene oxide and gold nanoclusters on an ITO electrode for studying the release of H2O2 from SH-SY5Y cells and for evaluation of drug-induced cell damage
A colorimetric and fluorescent pH probe was designed by doping carbon dots (C-dots) with Eu(III), Tb(III) and 2,6-pyridinedicarboxylic acid (DPA). The resulting nanoparticles were applied as fluorescent indicators for pH values (best detected at excitation/emission wavelengths of 272/545, 614 nm). The pH induced optical effects are due to pH induced variations in energy transfer. The fluorescence of the probe shows a continuous color variation, and a linear change with pH values in the range from 3.0 to 10.0 can be established by using a Commission Internationale de L’Eclairage (CIE) chromaticity diagram. This new kind of pH nanoprobe is more accurate than previously reported pH indicator probes because the pH value can be calculated by using chromaticity coordinates that only depend on the chromaticity. The pH nanoprobe was applied to visualize pH values in human breast adenocarcinoma cells (MCF-7).
Graphical abstract Carbon dots modified with Eu(III) and Tb(III) complexes of 2,6-pyridinedicarboxylic acid (DPA) were prepared. The doped carbon dots were used as a pH-sensitive nanosensor. The fluorescence chromaticity of the nanoparticles changes with the variation of pH value.
A magnetic glassy carbon electrode (mGCE) was modified with a ternary composite prepared from Prussian blue (PB), magnetite (Fe3O4) nanoparticles, and reduced graphene oxide (rGO) in order to obtain an amperometric sensor for hydrazine. The utilization of Fe3O4 facilitates the magnetic immobilization and separation of sensing material, while the use of rGO enhances sensitivity. The surface coverage and the stability of the PB on the modified electrode were considerably improved. The electro-oxidative response to hydrazine was investigated with this modified mGCE using cyclic voltammetry and amperometric. The sensor, typically operated at a voltage of 0.2 V (vs. SCE), displays superior response hydrazine, with a response time of 4 s, a sensitivity of 97.73 μA μM?1 cm?2 and a 13.7 nM detection limit.
Graphical abstract A magnetic glassy carbon electrode was modified with a ternary composite prepared from Prussian blue, magnetite nanoparticles, and reduced graphene oxide to obtain a selective amperometric sensor for dissolved hydrazine.
Three ferrites of type MFe2O4 (where M is bivalent Fe, Co or Mn) dispersed on multi-walled carbon nanotubes (MWCNTs) were prepared by a coprecipitation method. Their electrocatalytic properties toward the reduction of H2O2 at pH 7.4 were systematically compared. Catalytic reduction rates at an applied potential of ?0.4 V (vs. Ag/AgCl) and pseudo Michaelis-Menten constants show the electrocatalytic ability to follows the order Fe3O4 > CoFe2O4 > MnFe2O4. This diversity is attributed to the differences in the M(II) used and its occupancy on the lattice surface. The sensitivities are 120.98 ± 0.15, 48.45 ± 0.23 and 32.25 ± 0.27 μA cm?2 mM?1, and the limits of detection are 0.98, 2.59 and 5.64 μM of H2O2 (at an S/N ratio of 3).
Graphical abstract The activity diversity of MFe2O4 originates from the differences of the M(II) substitution and its occupancy on the lattice surface. Moreover, a process of electrochemical sensing of H2O2 is illustrated.
A SERS-based aptasensor for ochratoxin A (OTA) is described. It is making use of Fe3O4@Au magnetic nanoparticles (MGNPs) and of Au@Ag nanoprobes modified with the Raman reporter 5,5-dithiobis-(2-nitrobenzoic acid; DTNB). Au-DTNB@Ag NPs were modified with the OTA aptamer (aptamer-GSNPs) and used as Raman signal probes. The SERS peak of DTNB at 1331 cm?1 was used for quantitative analysis. MGNPs modified with cDNA (cDNA-MGNPs) were used as capture probes and reinforced substrates. When the Au-DTNB@Ag-Fe3O4@Au complexes are formed through oligonucleotide hybridization, the Raman signal intensity of the Raman probe is significantly enhanced. If the OTA concentration in samples increases, more Raman signal probes (aptamer-GSNPs) will dissociate from the cDNA-MGNPs because more OTA aptamer is bound by OTA. This leads to a lower Raman signal after magnetic separation. Under the optimal conditions, the detection limit for OTA is 0.48 pg·mL?1 based on 3σ criterion. This is attributed to the multiple Raman signal enhancement and the good performance of the OTA aptamer. The good recovery and accuracy of the assay was confirmed by evaluating spiked samples of wine and coffee.
Graphical abstract Schematic of an aptamer based SERS assay for OTA by integrating Fe3O4@AuNPs (MGNPs) with Au-DTNB@Ag NPs with multiple signal enhancement. Aptamer modified Au-DTNB@Ag NPs are used as Raman probes, and MGNPs modified with cDNA are used as capture probes and reinforced substrates.
The authors introduce an arc ion plating method for the deposition of chromium oxide (Cr2O3) on a steel wire substrate, and its use as a coating for solid phase microextraction. The coating has a micro- and nano-scaled structure after annealing at 700 °C. It is found that Cr2O3 exhibits a good extraction capability for the aromatic hydrocarbons naphthalene, anthracene, fluorene, fluoranthene, and biphenyl. Following desorption by high temperature at 300 °C, the analytes were quantified by gas chromatography (GC). The limits of detection are in the range between 20 and 200 ng·L?1, and calibration plots are linear within a wide range (0.2 to 400 μg·L?1). The coating has excellent mechanical properties, with a hardness is as high as 31.7 GPa, and the adhesion strength between coating and substrate reaches 20.1 N (corresponding to the critical Hertzian contact stress of 10 GPa). This, along with the chemical and thermal stability of the Cr2O3 coating, endows the wire with a long operational life. It was used for at least 100 times without any obvious decline of extraction capability.
Graphical abstract An arc ion plating method was introduced for the deposition of chromium oxide (Cr2O3) on a steel wire substrate, and its use as a coating for solid phase microextraction with high mechanical strength, stability, and long operational lifetime.
An F0F1-ATPase-based aptasensor is described for the fluorometric determination of Vibrio parahaemolyticus. Chromatophores containing F0F1-ATPases were first prepared from Rhodospirillum rubrum cells. Then, an aptamer-functionalized chromatophore acts as the capture probe, and a chromatophore labeled with the pH probe fluorescein acts as the signalling probe. In the presence of V. parahaemolyticus, the rotation rate of F0F1-ATPase is decreased due to the formation of the aptamer-chromatophore complex. This leads to a retarded proton flux out of the chromatophores. As a result, the pH value inside the chromatophores is reduced, and the fluorescence of the pH probe F1300 is accordingly decreased. The relative fluorescence varies linearly over the 15 to 1.5?×?106 cfu·mL?1Vibrio parahaemolyticus concentration range, and the limit of detection is 15 cfu·mL?1. The method was applied to analyze artificially contaminated salmon samples where it showed excellent perfomance.
Graphical abstract In this assay, aptamer functionalized chromatophores act as a capture probe, and the fluoresce in labeled chromatophores as signalling probe. The formation of aptamer-chromatophore complex leads to a retarded proton flux out of the chromatophores. As a result, the pH value inside the chromatophores is reduced, and fluorescence intensity is accordingly decreased.
An affinity-based protocol is described for the detection of Staphylococcus aureus (S. aureus). It is utilizing teicoplanin-functionalized magnetic beads as carriers. Teicoplanin, which binds to the walls of cells of S. aureus via five hydrogen bonds, acts as the recognition agent. Captured S. aureus is magnetically separated from the sample matrix and then specifically lysed by lysostaphin which cleaves the cross-linking pentaglycine bridges of peptidoglycan in the cell wall. Lastly, S. aureus is quantified via the inhibitory effect of released intracellular catalase on a chemiluminescent (CL) system composed of peroxidase, luminol, H2O2 and p-iodophenol because catalase decomposes H2O2. S. aureus can be detected with CL response in the 140 to 1.4?×?107 CFU·mL?1 concentration range and a detection limit as low as 47 CFU·mL?1 at a signal-to-noise ratio of 3. The method was evaluated by analyzing spiked samples including milk, human urine and saline injection solutions. The reliability was demonstrated by a recovery test and by comparison with a conventional plate counting method.
Graphical abstract An antibiotic-affinity protocol is developed to detect Staphylococcus aureus (S. aureus) by utilizing teicoplanin-functionalized magnetic beads (Teic-MBs) as carriers. S. aureus can be quantified by measuring the inhibition of luminol chemiluminescence (CL) signal by intracellular catalase.
