Highly selective and sensitive fluorescence turn-on probe for proline

A weakly fluorescent coumarinyl aldehyde was transformed into a strongly fluorescent aldol product by a catalytic amount of proline. The aldehyde probe has shown a highly selective fluorescence turn-on response toward proline over other amino acids with micromolar sensitivity.     

Selective turn-on fluorescence detection of cyanide in water using hydrophobic CdSe quantum dots

The ability of 2,2'-bipyridine-bound copper(ii) ions to quench the photoluminescence of hydrophobic CdSe quantum dots is used to create a novel, selective turn-on fluorescence cyanide sensor.     

A fluorescence turn-on H2O2 probe exhibits lysosome-localized fluorescence signals

A new fluorescence turn-on probe that responds exclusively to H(2)O(2) exhibits subcellular localized fluorescence staining of lysosomes.     

A turn-on fluorescent probe for selective and sensitive detection of hydrogen sulfide

An imidazolethione based turn-on fluorescent probe was synthesized for the detection of hydrogen sulfide, a biologically relevant molecule and an important air pollutant. The probe rapidly and selectively reacted with hydrogen sulfide to produce a strongly fluorescent product, resulting in the fluorescence enhancement of the system. The detection limit was determined to be 30 nM at the probe concentration of 1.0 μM. An indicating paper for visual detection of hydrogen sulfide gas has been fabricated by immobilizing the probe on a piece of appropriate paper substrate, and the detection limit of the visual method reached as low as 0.7 ppm. Moreover, the fluorescence turn-on/off of the system showed good reversibility when exposed alternately to hydrogen sulfide and mercuric ion, which was utilized to make an INHIBIT logic circuit for the presence of the two species.     

Highly sensitive naked-eye and fluorescence "turn-on" detection of Cu(2+) using Fenton reaction assisted signal amplification

Increase of pH induced by Cu(2+)-catalyzed Fenton reaction promoted ring-opening of triazole-linked fluorescein lactone, which enabled selective "turn-on" fluorescent detection of Cu(2+), along with ultralow naked-eye detection limit down to 200 nM.     

A sensitive and selective detection method for thiol compounds using novel fluorescence probe

In this work, a sensitive and selective detection method based on fluorescence resonance energy transfer (FRET) was developed for analyzing thiol compounds by using a novel fluorescent probe. The new fluorescent probe contains a disulfide bond which selectively reacts with nucleophilic thiolate through the thiol-disulfide exchange reaction. An obvious fluorescence recovery can be observed upon addition of the thiol compound in the fluorescent probe solution due to the thiol-disulfide exchange reaction and the destruction of FRET. This novel probe was successfully used to determine dithiothreitol (DTT), glutathione (GSH) and cysteine (Cys). The limits of detection (LOD) were 2.0 μM for DTT, 0.6 μM for GSH, and 0.8 μM for Cys. This new detection method was further investigated in the analysis of compound amino acid injection.     

Selective and sensitive fluorescence turn-on Zn~(2+) probes based on combination of anthracene,diphenylamine and dipyrrin

Two fluorescence turn-on Zn~(2+) probes were developed by introducing an anthracenyl fluorophore through the linkage of a diphenylamino moiety at the 5-position of a dipyrrin moiety.Thus,two compounds with weak fluorescence were designed,synthesized,and employed as CHEF(chelation enhanced fluorescence) type fluorescence turn-on Zn~(2+) probes,which exhibit dramatic fluorescence enhancement upon addition of Zn~(2+),showing high sensitivities and impressive detection limits of 13 and12 nM,respectively,better than their analogues containing simple aryl substituents at the 5 positions of a di-or tripyrrin moiety.In addition,both of the probes exhibit good selectivity,short response time of less than 10 s and wide applicable pH ranges.Furthermore,the weak fluorescence nature of the probes was rationalized based on viscosity dependence measurements and theoretical calculations.These results provide further insight into the development of selective and sensitive zinc probes.     

Label free fluorescence turn-on detection of polynucleotide kinase activity with a perylene probe

A single stranded oligonucleotide could induce aggregation of a perylene probe, the probe's monomer fluorescence was efficiently quenched. However, when the oligonucleotide was 5'-phosphorylated by polynucleotide kinase, it could be very efficiently degraded by lambda exonuclease, probe monomers were released, and a turn on fluorescence signal was detected.     

Label-free fluorescence turn-on detection of microRNA based on duplex-specific nuclease and a perylene probe

A novel fluorescence turn-on microRNA (miRNA) detection method based on duplex-specific nuclease (DSN) and a perylene probe is presented in this study. A positively charged perylene derivative (compound 1) was used as the fluorescent probe. Compound 1 exhibits strong monomer fluorescence in an aqueous buffer solution. It is well known that single-stranded DNA is a polyanion in nature. Thus, it can induce the aggregation of compound 1 through strong electrostatic, hydrophobic and π−π stacking interactions. As a result, the fluorescence of compound 1 was efficiently quenched. When the target miRNA was added, the formation of DNA-RNA hybridized duplex initiated the cleavage of the DNA strand by DSN cycle reaction, which resulted in disaggregation of compound 1. A fluorescence turn-on signal was detected, and a novel miRNA sensing method was therefore established. The presented method is label-free, simple, cost effective, sensitive and selective.     

A sensitive graphene oxide-DNA based sensing platform for fluorescence "turn-on" detection of bleomycin

A sensitive and selective fluorescent sensing platform for bleomycin (BLM) was developed based on BLM-induced DNA strand scission and the difference in affinity of graphene oxide for single-stranded DNA containing different numbers of bases in length.     

A novel rhodamine-based turn-on probe for fluorescent detection of Au3+ and colorimetric detection of Cu2+

In this work, we design and synthesize the novel probe RC through introduction the 1-aza-4,13-dithia-15-crown-5 ring into the structure of rhodamine 6G hydrazide, where the N atom of crown ring is responsible for quenching of rhodamine fluorescence. The compound obtained behaves as multifunctional cation sensor providing selective fluorescent response to Au³⁺ and selective colorimetric response to Cu²⁺ ions in aqueous acetonitrile (1/1, v/v) at pH 7.0. The use of 10^?5?M RC solution allowed reliable determination of target cations in the presence of a wide range of environmentally relevant ions with detection limits of 2?×?10^?6?M and 5?×?10^?7?M for gold and copper, respectively.     

Selective fluorescence turn-on of a prefluorescent azomethine with Zn

A prefluorescent conjugated azomethine (4) was prepared by condensing 8-hydroxyquinoline-5-carbaldehyde with 2-amine thiophene. The fluorescence of the azomethine was quenched in organic solvents including dichloromethane, methanol, DMSO, and DMF. However, the fluorescence of 4 was selectively revived in the presence of zinc and an absolute quantum yield Φ_fl = 0.15 was measured.     

A highly selective and sensitive fluorescence "turn-on" probe for Ag+ in aqueous solution and live cells

A naphthalimide-based fluorescent probe, NPQ, that contains a novel receptor was successfully developed. NPQ exhibited "turn-on" fluorescence and excellent selectivity toward Ag(+) in the presence of various other metal ions in aqueous solution. A series of control compounds were designed and synthesized in order to explore the photoinduced electron transfer (PET) quenching mechanism of NPQ and binding mode of NPQ with Ag(+). Moreover, with the NPQ-Ag(+) complex, I(-) was easily selectively recognized by a marked fluorescence quenching. The live cell imaging experiments demonstrate that NPQ can be used as a fluorescent probe for monitoring Ag(+) in living cells.     

A Schiff base fluorescence probe for highly selective turn-on recognition of Zn2+

A simple Schiff base CTS, synthesized between 2-hydroxy-1-naphthaldehyde and 2-benzylthio-ethanamine, was found to be a good turn-on fluorescence probe for the detection of Zn²⁺, due to the restriction of the rotation of the bond between CN and naphthalene ring and/or the blocking of the photo-induced electron transfer (PET) mechanism of the nitrogen atom to naphthalene ring. Excellent selectivity for Zn²⁺ was evidenced, over many other competing ions, including Fe³⁺, Cr³⁺, Ni²⁺, Co²⁺, Fe²⁺,Mn²⁺, Ca²⁺, Hg²⁺, Pb²⁺, Cu²⁺, Mg²⁺, Ba²⁺, Cd²⁺, Ag⁺, Li⁺, K⁺, and Na⁺, in EtOH/HEPES buffer (95:5, v/v, pH = 7.4). It was noteworthy that Cd²⁺ had no interference with Zn²⁺. The stoichiometric complex of CTS-Zn²⁺ was determined to be 2:1 for CTS and Zn²⁺ in molar, based on the Job plot and single crystal X-ray diffraction data. The binding constant of the complex was 85.7 M^?2 with a detection limit of 5.03 × 10^?7 M. The fluorescence bio-imaging capability of CTS to detect Zn²⁺ in live cells was also studied. These results indicated that CTS could serve as a favorable probe for Zn²⁺.     

Cytidine-stabilized gold nanocluster as a fluorescence turn-on and turn-off probe for dual functional detection of Ag and Hg

In this study, we have developed a label-free, dual functional detection strategy for highly selective and sensitive determination of aqueous Ag⁺ and Hg²⁺ by using cytidine stabilized Au NCs and AuAg NCs as fluorescent turn-on and turn off probes, respectively. The Au NCs and AuAg NCs showed a remarkably rapid response and high selectivity for Ag⁺ and Hg²⁺ over other metal ions, and relevant detection limit of Ag⁺ and Hg²⁺ is ca. 10 nM and 30 nM, respectively. Importantly, the fluorescence enhanced Au NCs by doping Ag⁺ can be conveniently reusable for the detection of Hg²⁺ based on the corresponding fluorescence quenching. The sensing mechanism was based on the high-affinity metallophilic Hg²⁺–Ag⁺ interaction, which effectively quenched the fluorescence of AuAg NCs. Furthermore, these fluorescent nanoprobes could be readily applied to Ag⁺ and Hg²⁺ detection in environmental water samples, indicating their possibility to be utilized as a convenient, dual functional, rapid response, and label-free fluorescence sensor for related environmental and health monitoring.     

Highly sensitive rare cell detection based on quantum dot probe fluorescence analysis

This study presents an efficient and sensitive method for detecting rare cells without cell culture, in which cells are analyzed quantitatively using quantum dots (QDs) as a fluorescent probe. By the conjugation of QDs with cells, the biotin–streptavidin reaction functions as a bridge to connect QDs and cells. The cells can be quantified based on the correlation of the QD fluorescence intensity with the cell population. Non-specific adsorption and cross-reaction of QD625–streptavidin on T cell membrane are neglected by reacting with biotin anti-human CD3 and mixing with red blood cell, respectively. Additionally, the photo-activation period and pH can be controlled to enhance the fluorescence of cell populations, which increases linearly with the number of T cells from 40 to 100,000, not only in a single T cell line but also in mixing with a total of 10⁶ red blood cells. Moreover, the specific T cells can be detected in less than 15 min, even though rare specific cells may number only 40 cells. Among the advantages, the proposed system for detecting rare cells include simplicity of preparation, low cost, rapid detection, and high sensitivity, all of which can facilitate the detection of circulating tumor cells in early stages of diagnosis or prognosis.      

Facile, sensitive and selective fluorescence turn-on detection of HSA/BSA in aqueous solution utilizing 2,4-dihydroxyl-3-iodo salicylaldehyde azine

A novel fluorescence turn-on detection method of human serum albumin (HSA) and bovine serum albumin (BSA) in aqueous solution is investigated using 2,4-dihydroxyl-3-iodo salicylaldehyde azine (DISA). Upon the addition of DISA to HSA/BSA solution, a fluorescence turn-on effect at 529 nm can be observed with a large stokes shift of ∼129 nm based on hydrophobic binding-mode between protein and dye. Under the optimal condition, the linear ranges of fluorescence intensity for HSA and BSA are 0.1-30 μg mL⁻¹ with the relative correlation coefficient of R² = 0.991 (n = 10) and 0.3-50 μg mL⁻¹ with R² = 0.997 (n = 10); and the detection limits for HSA and BSA based on IUPAC (C_DL = 3S_b/m) are 20 ng mL⁻¹ and 50 ng mL⁻¹, respectively.     

A fluorescence turn-on probe for the detection of thiol-containing amino acids in aqueous solution and bioimaging in cells

A turn-on fluorescent probe, based on a water-soluble terphenyl derivative, for the detection of cysteine and homocysteine is reported. The aldehyde groups in the probe play crucial roles in providing reaction with thiol groups in the amino acids, leading to a formation of thiazolidine (from cysteine) or thiazinane ring (from homocysteine). As a result, the new formation of such rings alters the electronic property of the conjugated system in the probe and results in emission enhancement. The probe in aqueous solution exhibits a remarkable increase in its quantum yield upon exposure to cysteine (up to 20-fold) and to homocysteine (up to 700-fold), while slight quenching is observed in the presence of glutathione. Moreover, an investigation on time-resolved fluorescence spectra of the probe in the presence of cysteine and homocysteine reveals potential discriminatory detection of cysteine and homocysteine. Bioimaging of the thiols in live HeLa cells was successfully applied.     

Chemoselective detection of Ag+ in purely aqueous solution using fluorescence ‘turn-on’ probe based on crown-containing 4-methoxy-1,8-naphthalimide

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