The article describes a method for rapid and visual determination of Hg(II) ion using unmodified gold nanoparticles (Au-NPs). It involves the addition of Au-NPs to a solution containing Hg(II) ions which, however, does not induce a color change. Next, a solution of lysine is added which induces the aggregation of the Au-NPs and causes the color of the solution to change from wine-red to purple. The whole on-site detection process can be executed in less than 15 min. Other amines (ethylenediamine, arginine, and melamine) were also investigated with respect to their capability to induce aggregation. Notably, only amines containing more than one amino group were found to be effective, but a 0.4 μM and pH 8 solution of lysine was found to give the best results. The detection limits for Hg (II) are 8.4 pM (for instrumental read-out) and 10 pM (for visual read-out). To the best of our knowledge, this LOD is better than those reported for any other existing rapid screening methods. The assay is not interfered by the presence of other common metal ions even if present in 1000-fold excess over Hg(II) concentration. It was successfully applied to the determination of Hg(II) in spiked tap water samples. We perceive that this method provides an excellent tool for rapid and ultrasensitive on-site determination of Hg(II) ions at low cost, with relative ease and minimal operation.
Rapid and ultrasensitive detection of mercury ions using gold nanoparticle based label-free colorimetric method with excellent sensitivity, easy operation and low cost.
An ultrasensitive conformation-dependent colorimetric assay has been developed for the detection of mercury(II) ions. It is based on the use of exonuclease III (Exo III)-assisted target recycling and gold nanoparticles (AuNPs). In the absence of Hg(II), the hairpin-shaped DNA probe (H-DNA) binds to AuNPs and stabilizes them in solutions of high ionic strength. In the presence of Hg(II), on the other hand, the sticky termini of the H-DNA form a rigid DNA duplex stem with a blunt 3′-terminus. Thus, Exo III is activated as a biocatalyst for selective and stepwise removal of mononucleotides from the 3′-terminus of the H-DNA. As a result, Hg(II) is released from the T?Hg(II)?T complexes. The guanine-rich sequences released from the H-DNA are then self-assembled with potassium ion to form a stable G-quadruplex conformation. In solutions of high ionic strength, this results in aggregation of AuNPs and a color change from red to blue which can be seen with bare eyes. The method is highly sensitive and selective. It has a linear response in the 10 pM to 100 nM Hg(II) concentration range, and the detection limit is as low as 3.2 pM (at an S/N ratio of 3). The relative standard deviation at a level of 0.5 nM of Hg(II) is 4.9% (for n?=?10). The method was applied to the detection of Hg(II) in spiked environment water samples, with recoveries ranging from 92% to 106%.
Graphical abstract A conformation-dependent colorimetric system was fabricated for label-free detection of mercury(II) by utilizing exonuclease III(Exo III)-assisted target recycling and gold nanoparticles (AuNPs).
A simple and reliable colorimetric method for determination of phthalates is developed utilizing uridine-5'-triphosphate (UTP)-modified gold nanoparticles as a color indicator and Cu(2+) as a cross-linker. The method demonstrates superior sensitivity with a detection limit of phthalates of ca. 0.5 ppm. 相似文献
In this study, we developed a fluorescence assay for the highly sensitive and selective detection of Hg2+ and Pb2+ ions using a gold nanoparticle (Au NP)-based probe. The Hg–Au and Pb–Au alloys that formed on the Au NP surfaces allowed the Au NPs to exhibit peroxidase-mimicking catalytic activity in the H2O2-mediated oxidation of Amplex UltraRed (AUR). The fluorescence of the AUR oxidation product increased upon increasing the concentration of either Hg2+ or Pb2+ ions. By controlling the pH values of 5 mM tris–acetate buffers at 7.0 and 9.0, this H2O2–AUR–Au NP probe detected Hg2+ and Pb2+ ions, respectively, both with limits of detection (signal-to-noise ratio: 3) of 4.0 nM. The fluorescence intensity of the AUR oxidation product was proportional to the concentrations of Hg2+ and Pb2+ ions over ranges 0.05–1 μM (R2 = 0.993) and 0.05–5 μM (R2 = 0.996), respectively. The H2O2–AUR–Au NP probe was highly selective for Hg2+ (>100-fold) and Pb2+ (>300-fold) ions in the presence of other tested metal ions. We validated the practicality of this simple, selective, and sensitive H2O2–AUR–Au NP probe through determination of the concentrations of Hg2+ and Pb2+ ions in a lake water sample and of Pb2+ ions in a blood sample. To the best of our knowledge, this system is the first example of Au NPs being used as enzyme-mimics for the fluorescence detection of Hg2+ and Pb2+ ions. 相似文献
Colorimetric detection of mercury ions (Hg(2+)) with the naked eye was accomplished within 1 min by a combination of non-crosslinking aggregation of double-stranded DNA-carrying gold nanoparticles and complex formation of thymine-Hg(2+)-thymine. 相似文献
A new approach for simple and rapid colorimetric detection of Hg(2+) in aqueous solution is proposed based on Hg(2+)-induced aggregation of mononucleotides-stabilized gold nanoparticles. 相似文献
The authors describe a colorimetric method for the determination of Hg(II) ion. It is based on the color change from red to colorless as displayed by gold nanoparticle (AuNP) modified with thymine - rich DNA. Signal amplification is accomplished by free strand displacement recycling. In this strategy, Hg(II) unfolds the arch-trigger duplex due to the high affinity between Hg(II) and the thymines to form T-Hg(II)-T structures, thereby causing the release of trigger. The liberated trigger unfolds the hairpin structure of H1, and unfolded H1 further unfolds with H2. As a result, the H2 hairpin displaces trigger, and the released trigger unfolds another H1. This results in strong and enzyme-free strand displacement recycling amplification. The aggregation of DNA-AuNPs occurs in the presence of the duplex formed by hairpins H2 and H1. This results in a color change from red to colorless that can be visually observed. Under optimal conditions, the assay has a detection range over 4 orders of magnitude and a 3.4 nM detection limit. The assay is selective, sensitive, rapid and cost-effective. In our perception, it represents a useful platform for determination of Hg(II).
Graphical abstract Schematic presentation of the simple, rapid, low cost colorimetric detection of mercury(II) based on enzyme-free strand displacement amplification along with DNA-labeled AuNP.
A major challenge in the area of DNA detection is the development of rapid methods that do not require polymerase chain reaction
(PCR) amplification of the genetic sample. The PCR amplification step increases the cost of the assay, the complexity of the
detection, and the quantity of DNA required for the assay. In this context, methods that are able to perform DNA analyses
with ultrasensitivity have recently been investigated with the aim of developing new PCR-free detection protocols. Functionalized
gold nanoparticles have played a central role in the development of such methods. Here, possibilities offered by functionalized
gold nanoparticle in the ultrasensitive detection of DNA are discussed. The different functionalization protocols available
for gold nanoparticles and the principal DNA detection methods that are able to detect DNA at the femtomolar to attomolar
level are presented. 相似文献
We unveil a new homogeneous assay-using mercaptopropionic acid-modified Au nanoparticles in the presence of 2,6-pyridinedicarboxylic acid for the highly selective and sensitive detection of Hg(2+) ions. 相似文献
Contamination of the environment with heavy metal ions has been an important concern throughout the world for decades. Driven by the need to detect trace amounts of mercury in environmental samples, this article demonstrates for the first time that nonlinear optical (NLO) properties of MPA-HCys-PDCA-modified gold nanoparticles can be used for rapid, easy and reliable screening of Hg(II) ions in aqueous solution, with high sensitivity (5 ppb) and selectivity over competing analytes. The hyper Rayleigh scattering (HRS) intensity increases 10 times after the addition of 20 ppm Hg(2+) ions to modified gold nanoparticle solution. The mechanism for HRS intensity change has been discussed in detail using particle size-dependent NLO properties as well as a two-state model. Our results show that the HRS assay for monitoring Hg(II) ions using MPA-HCys-PDCA-modified gold nanoparticles has excellent selectivity over alkali, alkaline earth (Li(+), Na(+), K(+), Mg(2+), Ca(2+)), and transition heavy metal ions (Pb(2+), Pb(+), Mn(2+), Fe(2+), Cu(2+), Ni(2+), Zn(2+), Cd(2+)). 相似文献
We report a simple and sensitive aptamer-based colorimetric detection of mercury ions (Hg2+) using unmodified gold nanoparticles as colorimetric probe. It is based on the fact that bare gold nanoparticles interact
differently with short single-strand DNA and double-stranded DNA. The anti-Hg2+ aptamer is rich in thymine (T) and readily forms T–Hg2+–T configuration in the presence of Hg2+. By measuring color change or adsorption ratio, the bare gold nanoparticles can effectively differentiate the Hg2+-induced conformational change of the aptamer in the presence of a given salt with high concentration. The assay shows a linear
response toward Hg2+ concentration through a five-decade range of 1 × 10−4 mol L−1 to 1 × 10−9 mol L−1. Even with the naked eye, we could identify micromolar Hg2+ concentrations within minutes. By using the spectrometric method, the detection limit was improved to the nanomolar range
(0.6 nM). The assay shows excellent selectivity for Hg2+ over other metal cations including K+, Ba2+, Ni2+, Pb2+, Cu2+, Cd2+, Mg2+, Ca2+, Zn2+, Al3+, and Fe3+. The major advantages of this Hg2+ assay are its water-solubility, simplicity, low cost, visual colorimetry, and high sensitivity. This method provides a potentially
useful tool for the Hg2+ detection. 相似文献
It is critical to be able to detect and quantify Hg2+ ions under aqueous conditions with high sensitivity and selectivity. The technique presented herein provides a direct way for simple colorimetric visualization of Hg2+ ions in aqueous solution, based on the formation of gold nanoparticles through the Hg2+ catalyzed HAuCl4/NH2OH reaction. The outstanding selectivity and sensitivity result from the well-known amalgamation process that occurs between mercury and gold. The entire procedure takes less than 20 min. The limit of detection (2 ppb) shows excellent potential for monitoring ultralow levels of mercury in water samples. 相似文献
Two new highly selective colorimetric chemosensors for Hg2+, based on azobenzene and highly selective Hg2+‐promoted deprotection of a dithioacetal have been designed and synthesized. In the presence of as little as 20 μM Hg2+, the sensors change their color from light yellow to deep red, which can easily be observed by the naked eye. The underlying signaling mechanism is intramolecular charge transfer (ICT). The sensors have good selectivity for Hg2+ with respect to several common alkali, alkaline earth, and transition metal ions. Furthermore, they can be used for in‐the‐field measurements by virtue of a dipstick approach without any additional equipment. 相似文献
A simple colorimetric method for the detection of copper ions in water is described. This method is based on the 'click' copper(I)-catalyzed azide-alkyne cycloaddition reaction and its use in promoting the aggregation of azide-tagged gold nanoparticles by a dialkyne cross-linker is described. Nanoparticle cross-linking, evidenced as a colour change, is used for the detection of copper ions. The lowest detected concentration by the naked eye was 1.8 μM, with the response linear with log(concentration) between 1.8-200 μM. The selectivity relative to other potentially interfering ions was evaluated. 相似文献
A simple but highly sensitive colorimetric method was developed to detect cancer cells based on aptamer–cell interaction. Cancer cells were able to capture nucleolin aptamers (AS 1411) through affinity interaction between AS 1411 and nucleolin receptors that are over expressed in cancer cells, The specific binding of AS 1411 to the target cells triggered the removal of aptamers from the solution. Therefore no aptamer remained in the solution to hybridize with complementary ssDNA-AuNP probes as a result the solution color is red. In the absence of target cells or the presence of normal cells, ssDNA-AuNP probes and aptamers were coexisted in solution and the aptamers assembled DNA-AuNPs, produced a purple solution. UV–vis spectrometry demonstrated that this hybridization-based method exhibited selective colorimetric responses to the presence or absence of target cells, which is detectable with naked eye. The linear response for MCF-7 cells in a concentration range from 10 to 105 cells was obtained with a detection limit of 10 cells. The proposed method could be extended to detect other cells and showed potential applications in cancer cell detection and early cancer diagnosis. 相似文献
As(III) specifically interacts with an arsenic-binding aptamer to form an As(III)-aptamer complex, so that the following cationic polymer can aggregate gold nanoparticles (AuNPs) and cause a remarkable change in color, which enables the colorimetric detection of As(III) with high selectivity and a detection limit of 5.3 ppb. 相似文献
A DNA-Au NP probe for sensing Hg2+ using the formation of DNA-Hg2+ complexes through thymidine (T)-Hg2+ -T coordination to control the negative charge density of the DNA strands-thereby varying their structures-adsorbed onto Au NPs. 相似文献
