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.
A zinc(II)-responsive ratiometric fluorescent core-shell nanoprobe (referred to as QPNPs) is described. It consist of an optimized combination of an internal reference dye (TBAP) encapsulated in the core, and a Zn(II)-specific indicator dye (PEIQ) in the shell. The nanoprobe was synthesized via single-step graft copolymerization induced by tert-butyl hydroperoxide at 80 °C. QPNPs exhibit a well-defined core-shell nanostructure and well-resolved dual emissions after photoexcitation at 380 nm. After exposure to Zn(II), the QPNPs display a green fluorescence peaking at ~500 nm that increases with the concentration of Zn(II), while the pink fluorescence of the porphine-derived reference dye peaking at ~650 nm remains unchanged. This results in color change from pink to green and thus enables Zn(II) to be detected both spectroscopically and with bare eyes. Zn(II) can be quantified with a 3.1 nM detection limit. The core-shell structured nanoprobe was also applied to real-time imaging of Zn(II) in living HeLa cells and in zebrafish. This work establishes a reliable approach to synthesize ratiometric fluorescent nanoprobes. It enables such nanoprobes to be prepared also by those not skilled in nanomaterial synthesis.
Graphical abstract A zinc(II)-responsive core-shell nanoprobe (referred to as QPNP) is synthesized via single-step graft copolymerization. Zn(II) can be quantitated with a 3.1 nM detection limit by the QPNPs through ratiometric fluorescence strategy (PEIQ as the Zn(II) indicator and TBAP as the reference dye).
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.
Sensing of intracellular singlet oxygen (1O2) is required in order to optimize photodynamic therapy (PDT). An optical nanoprobe is reported here for the optical determination of intracellular 1O2. The probe consists of a porous particle core doped with the commercial 1O2 probe 1,3-diphenylisobenzofuran (DPBF) and a layer of poly-L-lysine. The nanoparticle probes have a particle size of ~80 nm in diameter, exhibit good biocompatibility, improved photostability and high sensitivity for 1O2 in both absorbance (peak at 420 nm) and fluorescence (with excitation/emission peaks at 405/458 nm). Nanoprobes doped with 20% of DPBF are best suited even though they suffer from concentration quenching of fluorescence. In comparison with the commercial fluorescent 1O2 probe SOSG, 20%-doped DPBF-NPs (aged) shows higher sensitivity for 1O2 generated at an early stage. The best nanoprobes were used to real-time monitor the PDT-triggered generation of 1O2 inside live cells, and the generation rate is found to depend on the supply of intracellular oxygen.
Graphical abstract A fluorescent nanoprobe featured with refined selectivity and improved sensitivity towards 1O2 was prepared from the absorption-based probe DBPF and used to real-time monitoring of the generation of intracellular 1O2 produced during PDT.
The authors report on the design of a new Förster resonance energy transfer (FRET) based ratiometric nanoprobe for the determination of arginine. The method is based on the inhibition of the efficiency of FRET in assemblies formed between CdTe quantum dots capped with mercaptopropionic acid (QD-MPA) acting as energy donor, and the dye Cresyl Violet (CV) that acts as an energy acceptor at pH 8. Addition of arginine causes a displacement of the CV by arginine on the surface of the QD/MPA. Hence, the FRET between QD/MPA and CV is interrupted and fluorescence emission of the donor (QD/MPA) is restored. Arginine selectively binds to the QD/MPA via electrostatic and hydrogen bonding interactions between guanidinium and carboxylate. Under optimum conditions, the ratio of the fluorescence emissions peaking at 575 and 620 nm (under 400 nm excitation) is linear in the 1 to 30 μM arginine concentration range, and the detection limit is 0.51 μM. The nanoprobe displays good selectivity over 14 other amino acids, many metal ions, glucose, and ascorbic, tartaric and citric acids. The fluorescent nanoprobe was successfully applied to the determination of arginine in pure and spiked real samples and gave good recoveries. Its good selectivity, sensitivity, low-cost and rapidity make the QD-dye assembly a suitable nanoprobe for the quantitation of arginine.
Graphical abstract Schematic of a FRET ratiometric nanoprobe for arginine. It is based on quantum dots acting as energy donors and Cresyl Violet acting as energy acceptor. The FRET process is interrupted by the addition of arginine which selectively interacts with carboxy groups via a guanidinium-carboxylate salt bridge.
The authors describe new bifunctional mesoporous silica nanoparticles (NPs) for specific targeting of tumor cells and for intracellular delivery of the cancer drug doxorubicin (DOX). Mesoporous silica nanoparticles (MSNPs) were coated with blue fluorescent N-graphene quantum dots, loaded with the drug DOX, and finally coated with hyaluronic acid (HA). Cellular uptake of the NPs with an architecture of the type HA-DOX-GQD@MSNPs enabled imaging of human cervical carcinoma (HeLa) cells via fluorescence microscopy. The cytotoxicity of the nanoparticles on HeLa cells was also assessed. The results suggest that the NPs are higher cytotoxicity effect and exert in living cell imaging ability. Compared to the majority of other drug nanocarrier systems, the one described here enables simultaneous DOX release and fluorescent monitoring.
Graphical abstract Schematic of the bifunctional mesoporous silica nanoparticles were obtained via the Stöber method, along with the doxorubicin loaded and the hyaluronic acid capped. The sensor shows good specificity and significant cytotoxicity effect on Hela cells. (TEOS: tetraethyl orthosilicate; GQDs: graphene quantum dots; DOX: doxorubicin; HA: Hyaluronic acid).
We report on a widely applicable approach for protein detection by using triple-helix DNA mediated CuInS2 quantum dot (QD) and graphene oxide (GO) nanocomposite. The CuInS2 QDs were coated with mercaptopropionic acid and then covalently linked to a hairpin aptamer against lysozyme (HLA). Single-stranded DNA (triple helix-forming oligonucleotide; THFO) readily absorbs on the surface of GO via π-stacking interaction, and this results in the formation of THFO-GO. If HLA-CuInS2 QDs are added to the THFO-GO system, the fluorescence of HLA-CuInS2 QDs (at excitation/emission wavelengths of 590/665 nm) is quenched. Lysozyme has a higher affinity for HLA than THFO. Therefore, in the presence of lysozyme, it will bind to the HLA-CuInS2 QD and displace the THFO-GO. This results in the restoration of fluorescence that is related to the concentration of lysozyme. The fluorescence of the QDs is turned on. The calibration plot is linear in the 0.01 to 1.8 ng·mL ̄1 concentration range, with a 3 pg·mL ̄1 detection limit (at a signal-to-noise ratio of 3). The method was also applied to study the inhibition of lysozyme by IvyEc. In our perception, this method has a wide scope in that it may become applicable to any protein for which an appropriate aptamer is available.
Graphical abstract A novel convenient and universal fluorescence nanoprobe for sensitive and selective detection of lysozyme and inhibitor screening was established using triple-helix DNA mediated CuInS2 QDs and GO nanocomposites
Nanocomposites consisting of gold nanoclusters and graphene oxide (AuNC/GO) were prepared and investigated with respect to the design of new sensors for hydrogen peroxide (H2O2). The AuNC/GO hybrid nanomaterials were deposited on a gold electrode by the layer-by-layer assembly method, where they showed enhanced photoelectrical and sensing properties. The presence of graphene oxide improves the photoinduced electron separation efficiency of the AuNCs, as well as the catalytic effect of AuNCs on the electroreduction of H2O2. Compared to an electrode modified with AuNCs only, the new electrodes display a more than ten-fold enhanced photocurrent at a working voltage of -500 mV (vs. Ag/AgCl), higher sensitivity for H2O2 (25.76 nA?mM?1), lower LOD (2 μM) and extended linear range (from 30 μM to 5 mM). The sensors were applied to the determination of H2O2 extracted from living human umbilical vein endothelial cells stimulated by angiotensin II.
Graphical abstract Graphene oxide (GO) not only improves the photoinduced charge separation efficiency of fluorescent gold nanoclusters (AuNCs) based photoelectrochemical sensors, but also enhances the catalytic property of AuNCs on the detection of hydrogen peroxide (H2O2).
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.
The authors report on a one-pot approach for synthesizing highly fluorescent protamine-stabilized gold nanoclusters. These are shown to be a viable nanoprobe for selective and sensitive fluorometric determination of lead(II) via quenching of fluorescence via Pb(II)-Au(I) interaction. Under optimized conditions, fluorescence measured at excitation/emission peaks of 300/599 nm drops in the 80 nM–15 μM lead(II) concentration range. The detection limit is 24 nM, and relative standard deviations (for n?=?11) at concentrations of 0.10, 4.0 and 15 μM are 1.6, 2.5 and 1.9%, respectively. The relative recoveries of added lead(II) in the water samples ranged from 97.9?±?2.29% to 101.2?±?1.83%.
Graphical abstract Lead(II) ions are found to be able to selectively and sensitively quench the fluorescence of the protamine-gold nanoclusters (PRT-AuNCs). Thereby, an inexpensive, selective and sensitive lead(II) assay was established.
Gold nanoclusters (AuNCs) protected with a bovine serum albumin (BSA) coating are known to emit red fluorescence (peaking at 650 nm) on photoexcitation with ultraviolet light (365 nm). On addition of Cu(II) ions, fluorescence is quenched because Cu(II) complexes certain amino acid units in the BSA chain. Fluorescence is, however, restored if pyrophosphate (PPi) is added because it will chelate Cu(II) and remove it from the BSA coating on the AuNCs. Because PPi is involved in the function of telomerase, the BSA@AuNCs loaded with Cu(II) can act as a fluorescent probe for determination of the activity of telomerase. A fluorescent assay was worked out for telomerase that is highly sensitive and has a wide linear range (10 nU to 10 fM per mL). The fluorescent probe was applied to the determination of telomerase activity in cervix carcinoma cells via imaging. It is shown that tumor cells can be well distinguished from normal cells by monitoring the differences in intracellular telomerase activity.
Graphical abstract Gold nanoclusters (AuNCs) protected by bovine serum albumin (BSA) and displaying red photoluminescence were prepared as fluorescent probe for the determination of telomerase activity and used for imaging of cervix carcinoma (HeLa) cells.
Carbon polymer dots (CPDs) were prepared by a one-pot aqueous synthetic route from ascorbic acid and diethylenetriamine at room-temperature. The CPDs under 350-nm excitation exhibit blue fluorescence peaking at 430 nm with a quantum yield of 47%. Other features include an average diameter of 5 nm, a fluorescence that is independent of the excitation wavelength, good water dispersibility and photostability, and excellent biocompatibility. The CPDs are shown to be viable fluorescent probes for ferric ion which acts as a strong quencher. The response to Fe(III) is linear in the 0.2 to 10 μM concentration range, and the detection limit is 0.1 μM. The probe was applied to the determination of Fe(III) in environmental waters and to intracellular imaging of ferric ions in HeLa cells.
Graphical abstract Carbon polymer dots (CPDs) are prepared from ascorbic acid and diethylenetriamine (DETA) at room-temperature (RT). The RT-CPDs exhibit excellent optical performance, biocompatibility and selectivity of quenching by ferric ions. This can be applied for determination and intracellular imaging of ferric ion.
Hydrothermal treatment of a mixture of ethylene diamine, phosphoric acid and citric acid under ambient pressure generates fluorescent carbon dots that are co-doped with phosphorus and nitrogen. These have features such as (a) both green fluorescence (peaking at 430 nm; 30% quantum yield) and red fluorescence (peaking at 500 nm, quantum yield 78%), (b) wavelength-dependent emission peaks, and (c) insensitivity to changes of pH values, dot concentration and ionic strength. The C-dots are useful for both fluorescent (FL) and photoacoustic (PA) imaging of living tissue. PA imaging warrants better spatial resolution and allows deeper tissues to be imaged compared to most optical imaging techniques. It is essential to assign a photoacoustic contrast agent as most of the diseases do not show a natural photoacoustic contrast in their early stage. The dually emitting C-dots are shown to be a useful contrast agent for PA and FL imaging of mice tumors. Intravenous administration of the C-dots resulted in strong signals in both PA and FL imaging.
Graphical abstract Photographs of the excitation wavelength-dependent fluorescence of P,N-doped C-dots obtained from ethylenediamine, phosphoric acid and citric acid. Intravenous administration of the C-dots resulted in strong signals in both photoacoustic (PA) and fluorescent (FL) imaging.
The authors describe a fluorometric aptamer based assay for adenosine triphosphate (ATP). It is based on the use of carbon dots (CDs) and graphene oxide (GO). The resultant CD-aptamer is adsorbed on the surface of GO via π-stacking and hydrophobic interaction, and the fluorescence of CD-aptamer is quenched via fluorescence resonance energy transfer (FRET) between CDs and GO. If ATP is present, it will bind to the aptamer and the CD-aptamer will be desorbed from GO. This will suppress FRET and the fluorescence of the CDs is restored. Under the optimal conditions and at typical excitation/emission wavelengths of 358/455 nm, the assay has a 80 pM detection limit and a linear range that extends from 0.10 to 5.0 nM concentrations of ATP. The method was successfully applied to the determination of ATP in yogurt samples. This method can also be conceivably applied to the detection of other analytes for which appropriate aptamers are available.
Graphical abstract Schematic of a novel fluorometric ATP assay based on the fluorescence resonance energy transfer (FRET) between aptamer modified carbon dots (CD-aptamer) and graphene oxide (GO). CD-aptamer was used as the energy donor and molecular recognition probe, and GO acted as energy acceptor. This assay exhibits high sensitivity and selectivity with a detection limit as low as 80 pM.
A method is described for the determination of the polarity of mixed organic solvents by using the fluorescent probe Hostasol Red (HR) desposited on the outer surface of nanosized zeolite L. Organic solvents and their mixtures can be roughly classified according to their polarity with bare eyes and fluorometrically. Emission peaks range from 520 to 640 nm. Some solvents act as quenchers. The method is studied with series of protic and nonprotic solvents, and with selected mixtures of organic solvents.
Graphical abstract The dye Hostalene Red adsorbed on nanosized zeolite shows strong fluorescence solvatochromism. This can be exploited to quickly assess the polarity of solvents and solvent mixtures.
The authors describe a method for synthesizing graphene oxide quantum dots (GOQDs) possessing orange fluorescence with emission wavelength that can be tuned over the range from 537 to 593 nm by variation of the excitation wavelength. The GOQD display peroxidase-mimicking catalytic activity. Specifically, they catalyze the oxidation of dopamine to produce 4-(2-aminoethyl)benzene-1,2-quinone (AQ) which is colored and can quench the fluorescence of GOQDs. However, quenching is reversed by addition of NADP+, but not by its reduced form (NADPH). Based on these findings, an assay was worked out to monitor enzymatic reactions involving NADP+. The method allows NADPH to be detected in the 2–175 μM concentration range, with a 0.6 μM detection limit.
Graphical abstract Schematic of a top-down method for synthesizing fluorescent graphene oxide quantum dots (GOQD) by chemical degrading, exfoliation and self-assembly of graphene oxide (GO). The GOQDs display peroxidase-like activity and can oxidize dopamine to form a colored quinone that quenches the fluorescence of the GOQDs. The quenching efficiency is reduced, however, in the presence of NADP+.
The authors describe three fluorescein-conjugated peptides generated by cell-phage display for use as a diagnostic probes for fluorescent detection and imaging of Salmonella enteritidis and Salmonella typhimurium. The authors also designed a polyvalent-directed peptide polymer synthesized with poly-D-lysine and bifunctional succinimidyl 3-(2-pyridyldithio)propionate with an affinity and sensitivity that is higher by more than an order of magnitude compared to single peptides due to multiple binding site interactions. In order to establish a diagnostic system for food poisoning, imaging analysis was performed using fluorescence microscopy. The limit of detection of the diagnostic system based on polyvalent directed peptide interaction is 102 colony-forming units per mL for Salmonella.
Graphical abstract Schematic of a fluorescent method for detection and imaging of Salmonella enteritidis and Salmonella typhimurium by using a fluorescein labeled polyvalent-directed peptide polymer (PDPP) with a high affinity and sensitivity as a diagnostic probe. The system uses a microplate reader and was applied to the detection of food poisoning.
The authors report on an efficient method for the voltammetric sensing of dopamine (DA) by using an electrode modified with alternating monolayers of graphene oxide (GO) and Titanium dioxide (TiO2) nanoparticles anchored GO nanosheets (NSs)). The as-prepared nanostructures were characterized by photoluminescence spectroscopy, powder X-ray diffraction, Raman spectroscopy, FT-IR spectroscopy, transmission electron microscopy, scanning electron microscopy, atomic force microscopy and Energy Dispersive X-ray Analysis (EDAX) techniques. The GO/TiO2 nanocomposite (NC) was deposited on a glassy carbon electrode (GCE), where it displayed an excellent electrocatalytic activity toward the oxidation of DA, owing to its excellent conductivity, high specific surface area, enhanced interfacial contact and more negative zeta potential. Figures of merit include (a) a fast response (5 s), (b) a wide linear range (between 0.2 and 10 μM of DA) (c) a particularly low detection limit (27 nM), (d) a working potential as low as 0.25 V (vs. Ag/AgCl) and (e) a sensitivity of 1.549 μA·μM?1·cm?2. The GO/TiO2/GCE exhibited excellent selectivity over the other interferences as revealed by the differential pulse voltammetric and amperometric studies. The analysis of spiked urine samples resulted in recoveries in the range of 96 to 106%, with RSDs between 3.8 and 5.2%.
Graphical abstract A GO/TiO2 (graphene oxide/titanium dioxide) nanocomposite (NC) was prepared and exploited as electrochemical probes in DA detection. It displays a low detection limit, wide linear range and excellent selectivity.
An ultrasensitive paper based lateral flow assay is described for rapid and simultaneous fluorometric detection of several β-agonists including clenbuterol and its chemical analogues (mabuterol, brombuterol, cimaterol, cimbuterol, bromchlorbuterol and banbuterol). A nonspecific monoclonal antibody (mAb) against clenbuterol and its analogues was prepared and employed in a competitive immunoassay where mAb conjugated to fluorescent nanoparticles and free β-agonists compete for the binding sites. This enables rapid screening for the 7 β-agonists in a single run that takes about 8 min. Detection limits for the seven β-agonists are <50 pg g?1 of pork. Recoveries ranged from 69.5% to 102.4%, and relative standard deviations were ±15%. The assay was applied to the analysis of both using spiked and unspiked pork for β-agonists, and the results compare well to those obtained by HPLC-MS.
Graphical abstract Schematic presentation of an ultra sensitive fluorescent nanoparticle based paper based assay for rapid detection of multi β-agonists in pork tissue.
The authors describe a fluorometric switch assay for microRNA (miRNA). It is based on nonenzymatic ligation-rolling circle amplification (NELRCA). A click chemistry-mediated functionalized linear template was prepared by self-cycling. It is capable of forming a modified circular template (MLT) with a triazole linkage for amplified agent. MiRNA can recognize a binding region of the MLT, activates the NELRCA, and converts into rolling circle amplification products (RCPs). Subsequently, the added FAM-labeled signal probes (FAM-SPs) can hybridize to the RCPs. This RCPs/FAM-SPs duplex is less adsorbed onto the graphene oxide (GO) so that fluorescence (best measured at excitation/emission wavelengths of 490/520 nm) increases. In contrast to classical GO-based adsorption and displacement sensing system, the designed hybridization and adsorption fluorescent switch-on platform can reduce the assay time, and improve the detection efficiency of target. Under optimal conditions, the sensing platform has a detection limit as low as 0.75 fM. It can well discriminate target miRNA from other kinds of miRNA. Conceivably, this method can be extended to the trace detection of other nucleic acid biomarkers, and simultaneous recognition of multiple targets, thereby improving the early clinical diagnostic accuracy of cancer.
Graphical abstract A hybridization and adsorption switch-on sensing system was fabricated on nonenzymatic ligation-rolling circle amplification. Modified circular template with 1,4-connect triazole linkage was adopted as an identified and amplified agent for high sensitive detection of microRNA.
