Selective colorimetric and fluorometric sensing of Cu(II) by iminocoumarin derivative in aqueous buffer

A new iminocoumarin based receptor L (C(27)H(26)N(4)OS) is synthesized with pyridyl and benzothiazolyl functionality. Synthesis of L is easy and it is isolated in good yield. L shows a selective and distinct color change from yellow to orange with Cu(2+) over Li(+), Na(+), Ca(2+), Mg(2+), Cr(2+), Mn(2+), Fe(2+), Co(2+), Ni(2+), Cu(2+), Zn(2+), Cd(2+), Pb(2+), and Ag(+) whereas a slight change in color is also observed in the case of Hg(2+) but L shows selective fluorescent quenching only in the presence of Cu(2+) in aqueous HEPES buffer (pH 7.0). The naked eye detection limit of Cu(2+) is determined at 2 μM whereas an emission experiment shows a lower detection limit at 200 nM. Selectivity studies of L in presence of 50 equivalents of other ion(s) by emission experiment show no interference toward the detection of 1 equivalent of Cu(2+). Both UV-Vis and fluorescence studies in the presence of Cu(2+)-salts of different counter anions with various sizes and shapes (Cl(-), ClO(4)(-), NO(3)(-), CF(3)SO(3)(-), SO(4)(2-) and BF(4)(-)) show almost similar spectral output in buffer media irrespective of the nature of the counter anions. The detailed UV-Vis and fluorescence titration experiments suggest the existence of both 1:1 and 2:1 (L:Cu(2+)) complexation stoichiometry and EPR study shows d(x(2)-y(2)) ground state of the Cu(II) centre in the complex. Furthermore the formation of a mononuclear [Cu(L)(CH(3)CN)].2ClO(4) complex and the flexible conformation of L in the solid state are confirmed by the single-crystal X-ray structural study.     

Highly sensitive and selective chemosensor for Cu2+ detection based on a N-propargyl rhodamine 6G-hydrazide derivative

A novel fluorescence "turn-on" probe for Cu2+ detection has been designed based on a Cu2+ triggered spirolactam ring-opening reaction.The synthetic probe is a double-responsive fluorescent and colorimetric Cu2+-specific sensor.In aqueous solution,it exhibits high selectivity and excellent sensitivity.With a significant color change visible to the naked eye at the concentration of 3 μM(ca.0.19 mg/L),about one magnitude lower than the WHO(World Health Organization) recommended level(2.0 mg/L) for Cu2+ ions in drinking water,the probe could be used to monitor Cu2+ ions in drinking water.     

A ratiometric fluorescent chemosensor for iron: discrimination of Fe2+ and Fe3+ and living cell application

A newly designed probe, 6-thiophen-2-yl-5,6-dihydrobenzo[4,5]imidazo-[1,2-c] quinazoline (HL(1)) behaves as a highly selective ratiometric fluorescent sensor for Fe(2+) at pH 4.0-5.0 and Fe(3+) at pH 6.5-8.0 in acetonitrile-HEPES buffer (1/4) (v/v) medium. A decrease in fluorescence at 412 nm and increase in fluorescence at 472 nm with an isoemissive point at 436 nm with the addition of Fe(2+) salt solution is due to the formation of mononuclear Fe(2+) complex [Fe(II)(HL)(ClO(4))(2)(CH(3)CN)(2)] (1) in acetonitrile-HEPES buffer (100 mM, 1/4, v/v) at pH 4.5 and a decrease in fluorescence at 412 nm and increase in fluorescence at 482 nm with an isoemissive point at 445 nm during titration by Fe(3+) salt due to the formation of binary Fe(3+) complex, [Fe(III)(L)(2)(ClO(4))(H(2)O)] (2) with co-solvent at biological pH 7.4 have been established. Binding constants (K(a)) in the solution state were calculated to be 3.88 × 10(5) M(-1) for Fe(2+) and 0.21 × 10(3) M(-1/2) for Fe(3+) and ratiometric detection limits for Fe(2+) and Fe(3+) were found to be 2.0 μM and 3.5 μM, respectively. The probe is a "naked eye" chemosensor for two states of iron. Theoretical calculations were studied to establish the configurations of probe-iron complexes. The sensor is efficient for detecting Fe(3+)in vitro by developing a good image of the biological organelles.     

Synthesis and application of imprinted polyvinylimidazole-silica hybrid copolymer for Pb2+ determination by flow-injection thermospray flame furnace atomic absorption spectrometry

A novel ion imprinted polyvinylimidazole-silica hybrid copolymer (IIHC) was synthesized and used as a selective solid sorbent for Pb(2+) ions preconcentration using an on-line solid phase extraction (SPE) system coupled to TS-FF-AAS. The ionic hybrid sorbent was prepared using 1-vinylimidazole and 3-(trimethoxysilyl)propylmethacrylate as monomers, Pb(2+) ions as template, tetraethoxysilane as reticulating agent and 2,2'-azobis-isobutyronitrile as initiator. The best on-line SPE conditions concerning sorption behavior, including sample pH (6.46), buffer concentration (9.0 mmol L(-1)), eluent (HNO(3)) concentration (0.5 mol L(-1)) and preconcentration flow rate (4.0 mL min(-1)), were optimized by means of full factorial design and Doehlert matrix. The analytical curve ranged from 2.5 to 65.0 μg L(-1) (r=0.999) with limit of detection of 0.75 μg L(-1); the precision (repeatability) calculated as relative standard deviation (n=10) was 5.0 and 3.6% for Pb(2+) concentration of 10.0 and 60.0 μg L(-1), respectively. From on-line breakthrough curve, column capacity was 3.5 mg g(-1). Preconcentration factor (PF), consumptive index (CI) and concentration efficiency (CE) were 128.0, 0.16 mL and 25.6 min(-1), respectively. The selective performance of the sorbent, based on relative selectivity coefficient, was compared to NIC (non imprinted copolymer) for the binary mixture Pb(2+)/Cd(2+), Pb(2+)/Cu(2+) and Pb(2+)/Zn(2+). The results showed that ion imprinted polyvinylimidazole-silica hybrid polymer had higher selectivity for Pb(2+) than NIC at 64.9, 16.0 and 8.8 folds. The developed method was successfully applied for highly sensitive and selective Pb(2+) determination in different kinds of water samples, parenteral solutions and urine. Accuracy was also assessed by analyzing certified reference fish protein (DORM-3) and marine sediment (MESS-3 and PACS-2) with satisfactory results.     

A gold nanorod based colorimetric probe for the rapid and selective detection of Cu2+ ions

A gold nanorod (AuNR) based colorimetric probe was reported for the rapid and selective detection of Cu(2+) ions. The probe was fabricated by functionalizing cysteine (Cys) onto AuNR (Cys-AuNR) with an aspect ratio of 2.3. The strong coordination of Cu(2+) with cysteine resulted in a stable Cys-Cu-Cys complex, and induced the aggregation of the colloidal nanorods along with a rapid colour change from blue-green to dark gray. Potential factors affecting the performance of the probe for the detection of Cu(2+) were carefully optimized, including the pH value of the buffer media, the concentration of cysteine, and the kinetics for the coordination of Cu(2+) with Cys-AuNR. Under optimal conditions, the developed colorimetric method gave a linear range of 1-100 μM for Cu(2+), and a detection limit (3s) of 0.34 μM. Moreover, the developed method exhibited excellent selectivity for Cu(2+), and quantitative spike-recoveries from 90% to 107% in environmental water samples. The proposed colorimetric approach can in principle be used to detect other metal ions by functionalizing various specific ligands onto the AuNR that can selectively bind the other target metal ions.     

Fluorimetric determination of copper(II) in aqueous solution using lucifer yellow CH as selective metal reagent

Lucifer yellow CH is shown to be a highly selective fluorescent reagent for the determination of Cu(III) in the microg L(-1) concentration range. The fluorophore is statically quenched by Cu(II); the carbohydrazide group was assigned as the complexing part of the dye molecule. A total range of Cu(II) determination from 0.06 mg L(-1) (1 micromol L(-1)) to 6.3 mg L(-2) (100 micromol L(-1)) with a limit of detection of 0.019 mg L(-1) (0.3 micromol L(-1)) was obtained, along with surprisingly high selectivity. There was no interference from alkaline and earth alkaline metal ions. The cross sensitivity to heavy metal ions was evaluated by the separate solution method and by competitive binding experiments. Calibration plots are shown for Cu(II) determination at different pH and the dissociation constant was determined. The application of the reagent was demonstrated by the determination of the Cu(II) content of tap water samples.     

Two-photon fluorescent probe for cadmium imaging in cells

A novel two-photon excited fluorescent probe for cadmium (named as TPCd) was designed and synthesized utilizing a prodan (6-acetyl-2-methoxynaphthalene) derivative as the two-photon fluorophore and an o-phenylenediamine derivative as the Cd(2+) chelator, which possessed favorable photophysical properties and good water-solubility. The probe was designed with a photoinduced electron transfer (PET) mechanism and thus was weakly fluorescent itself. After binding with Cd(2+) which blocked the PET process, the fluorescence intensity of the probe was enhanced by up to 15-fold under one-photon excitation (OPE) and 27-fold under two-photon excitation (TPE), respectively. The two-photon action cross-section (Φδ) of the TPCd-Cd complex at 740 nm reached 109 GM compared to 3.6 GM for free TPCd, indicating the promising prospect of the probe in two-photon application. TPCd chelated Cd(2+) with 1 : 1 stoichiometry, and the apparent dissociation constant (K(d)) was 6.1 × 10(-5) M for the one-photon mode and 7.2 × 10(-5) M for the two-photon mode. The probe responded to Cd(2+) over a wide linear range from 0.1 to 30 μM with a detection limit of 0.04 μM. High selectivity of the probe towards Cd(2+) was acquired in Tris-HCl/sodium phosphate buffer. The probe was pH-independent in the biologically relevant pH range and non-toxic to living cells at reasonable concentration levels, warranting its in vivo applications. Through two-photon microscopy imaging, the probe was successfully applied to detect Cd(2+) uptake in living HepG2 cells.     

A medium-controlled fluorescence dual-responsive probe for Cu2+ and Hg2+ in aqueous solutions

In this study, we report a histidine-based fluorescence probe for Cu(2+) and Hg(2+), in which the amino group and imino group were modified by two common protective groups, 9-fluorenylmethoxycarbonyl and trityl group, respectively. In a water/methanol mixed solution, the probe displayed a selective fluorescence "turn-off" response to Cu(2+) when the ratio of CH(3)OH/H(2)O was higher than 1:1. Specifically, when the solvent is changed to 1:1 methanol/water, the 304 nm fluorescence peak is enhanced, while the 317 nm peak is weakened, upon addition of either Cu(2+) or Hg(2+) ions. The mechanism for such distinct responses of the probe to Cu(2+) and Hg(2+) was further clarified by using NMR and molecular simulation. The experiment results indicated that the polarity of solvent could influence the coordination mode of 1 with Cu(2+) and Hg(2+), and control the fluorescence response as a "turn-off" or ratiometric probe.     

Fluorescent gold clusters as nanosensors for copper ions in live cells

This paper reports the use of fluorescent gold nanoclusters synthesized using bovine serum albumin (Au-BSA) for the sensing of copper ions in live cells. The fluorescence of the clusters was found to be quenched by Cu(2+) enabling its detection in cells. The selectivity of the nanosensor was demonstrated in the presence of several cations excluding Hg(2+). We did not study the effect of Hg(2+) since it was reported earlier. The present study suggests that Cu(2+) induced fluorescence quenching is due to its binding to BSA rather than the fluorescence quenching by metal-metal interaction as in the case of Hg(2+). The Au-BSA showed excellent selectivity to Cu(2+) at various pH conditions. The 'turn off' of fluorescence can be retrieved by a Cu(2+) chelator glycine. Our results showed that gold clusters can be used as a 'turn off' sensor for copper and a 'turn on' sensor for glycine. Under the experimental conditions, the probe showed a response for Cu(2+) over a range of 100 μM to 5 mM with a detection limit of 50 μM. The role of Cu(2+) in the misfolding and disassembly of Prion Protein (PrP) leading to various maladies is well ascertained. The methodology we reported here seems to be useful in supplementing other techniques in predicting disease conditions involving Cu(2+).     

Luminescent ruthenium probe for the determination of acetyl phosphate in complex biological matrices

The first probe for the fluorogenic determination of acetyl phosphate (AcP), (bpy)(2)Ru(1,10-phenanthroline-5,6-dione dioxime) (RuPDO), was prepared and its reaction with AcP was studied in detail. The emission of the weakly luminescent RuPDO is red shifted and strongly enhanced upon reaction with AcP in the presence of metal cations like Zn(2+) or Cu(2+). The reaction occurs within 60 min incubation time under highly biocompatible conditions (aqueous buffer of pH 7, 37 °C). A linear dynamic range from 10 to 200 μmol L(-1) is observed with an LOD of AcP of 3.4 μmol L(-1) (for RuPDO-Zn). Other bio-phosphates studied show only weak interference. Furthermore, the applicability of the probe in complex biological matrices was evaluated.     

Visible-near-infrared and fluorescent copper sensors based on julolidine conjugates: selective detection and fluorescence imaging in living cells

We present novel Schiff base ligands julolidine-carbonohydrazone 1 and julolidine-thiocarbonohydrazone 2 for selective detection of Cu(2+) in aqueous medium. The planar julolidine-based ligands can sense Cu(2+) colorimetrically with characteristic absorbance in the near-infrared (NIR, 700-1000 nm) region. Employing molecular probes 1 and 2 for detection of Cu(2+) not only allowed detection by the naked eye, but also detection of varying micromolar concentrations of Cu(2+) due to the appearance of distinct coloration. Moreover, Cu(2+) selectively quenches the fluorescence of julolidine-thiocarbonohydrazone 2 among all other metal ions, which increases the sensitivity of the probe. Furthermore, quenched fluorescence of the ligand 2 in the presence of Cu(2+) was restored by adjusting the complexation ability of the ligand. Hence, by treatment with ethylenediaminetetraacetic acid (EDTA), thus enabling reversibility and dual-check signaling, julolidine-thiocarbonohydrazone (2) can be used as a fluorescent molecular probe for the sensitive detection of Cu(2+) in biological systems. The ligands 1 and 2 can be utilized to monitor Cu(2+) in aqueous solution over a wide pH range. We have investigated the structural, electronic, and optical properties of the ligands using ab initio density functional theory (DFT) combined with time-dependent density functional theory (TDDFT) calculations. The observed absorption band in the NIR region is attributed to the formation of a charge-transfer complex between Cu(2+) and the ligand. The fluorescence-quenching behavior can be accounted for primarily due to the excited-state ligand 2 to metal (Cu(2+)) charge-transfer (LMCT) processes. Thus, experimentally observed characteristic NIR and fluorescence optical responses of the ligands upon binding to Cu(2+) are well supported by the theoretical calculations. Subsequently, we have employed julolidine-thiocarbonohydrazone 2 for reversible fluorescence sensing of intracellular Cu(2+) in cultured HEK293T cells.     

Relationship between the thermally induced reorientations of aromatic solvate molecules in Cu(hfac)2-nitroxide breathing crystals and the character of the magnetic anomaly

A new group of "breathing" crystals has been synthesized. These are aromatic solvates of the copper(II) hexafluoroacetylacetonate complex with spin-labeled pyrazole Cu(hfac)(2)L·0.5Solv, where L is 2-(1-butyl-1H-pyrazol-4-yl)-4,4,5,5-tetramethyl-4,5-dihydro-1H-imidazole-3-oxide-1-oxyl and Solv is benzene, toluene, ethylbenzene, propylbenzene, butylbenzene, styrene, o-xylene, m-xylene, p-xylene, 1,4-bis(trifluoromethyl)benzene, 1-methyl-4-ethylbenzene, 1-methyl-4-vinylbenzene, 1,4-diethylbenzene, 1,2,3-trimethylbenzene, or 1,2,4-trimethylbenzene. The main feature of Cu(hfac)(2)L·0.5Solv single crystals is their remarkable mechanical stability and ability to undergo thermally induced structural rearrangements accompanied by spin-crossover-like phenomena. The structures of Cu(hfac)(2)L·0.5Solv solvates are similar and based on mutually parallel {Cu(hfac)(2)L}(∞) heterospin chains with a "head-to-head" motif. The localization of voids with guest molecules being the same in all crystals, the temperature dependence of the effective magnetic moment (μ(eff)) for Cu(hfac)(2)L·0.5Solv is determined by the structure of the guest molecules, along which the polymer chains are "gliding" when the temperature changes. When the temperature decreased from 300 to 100-50 K, μ(eff) decreased, abruptly or gradually, from 2.7-2.4 to ~1.8 β for the majority of Cu(hfac)(2)L·0.5Solv except the solvates with benzene, toluene, and 1,4-bis(trifluoromethyl)benzene. When Cu(hfac)(2)L·0.5C(6)H(6) and Cu(hfac)(2)L·0.5CH(3)-C(6)H(5) were cooled to 50 K, μ(eff) decreased to ~2.1-2.2 β. When Cu(hfac)(2)L·0.5(1,4-(CF(3))(2)-C(6)H(4)) was cooled to 50 K, μ(eff) initially decreased from ~2.7 to 1.9 β and then abruptly increased to ~2.4 β. A single-crystal X-ray diffraction analysis of each solvate within a temperature range wider than the range of magnetic anomaly temperatures revealed a complex interrelated dynamics of the aromatic solvent guest molecules and heterospin chains. The dynamics largely depended on the orientation of the solvent guest molecules relative to the polymer chains. An analysis of the thermally induced phase transformations revealed a relationship between the structural rearrangement of Cu(hfac)(2)L·0.5Solv and the form of the magnetic anomaly on the μ(eff)(T) curve and between the structural rearrangement of the solvate and the temperature of the magnetic effect.     

基于香豆素与胍的荧光探针的合成及对Co2+、Fe3+的识别研究(英文)

本论文设计合成了基于1,3-二氨基胍盐酸盐、氨基胍盐酸盐的新型香豆素类荧光探针L1、L2。通过紫外-可见、荧光光谱的变化研究探针L1、L2对金属离子的识别效应。利用Job’s plot曲线确定探针L1与Co²⁺形成了1∶2的配合物,探针L2和Fe³⁺形成了3∶1的配合物,且表现为明显的荧光增强。探针L1对Co²⁺的检出限可达到10^-6mol/L,探针L2对Fe³⁺的检出限可达到10^-7mol/L。两种高灵敏度荧光探针有望应用于生物和环境监测领域。     

Visual detection of copper(II) ions in blood samples by controlling the leaching of protein-capped gold nanoparticles

We have developed a simple, low-cost, paper-based probe for the selective colorimetric detection of copper ions (Cu(2+)) in aqueous solutions. The bovine serum albumin (BSA)-modified 13.3-nm Au nanoparticle (BSA-Au NP) probe was designed to detect Cu(2+) ions using lead ions (Pb(2+)) and 2-mercaptoethanol (2-ME) as leaching agents in a glycine-NaOH (pH 12.0) solution. In addition, a nitrocellulose membrane (NCM) was used to trap the BSA-Au NPs, leading to the preparation of a nanocomposite film consisting of a BSA-Au NP-decorated membrane (BSA-Au NPs/NCM). The BSA-Au NPs probe operates on the principle that Cu deposition on the surface of the BSA-Au NPs inhibits their leaching ability, which is accelerated by Pb(2+) ions in the presence of 2-ME. Under optimal solution conditions (5 mM glycine-NaOH (pH 12.0), Pb(2+) (50 μM), and 2-ME (1.0 M)), the Pb(2+)/2-ME-BSA-Au NPs/NCM enabled the detection of Cu(2+) at nanomolar concentrations in aqueous solutions by the naked eye with high selectivity (at least 100-fold over other metal ions). In addition, this cost-effective probe allowed for the rapid and simple determination of Cu(2+) ions in not only natural water samples but also in a complex biological sample (in this case, blood sample).     

An integrated portable Raman sensor with nanofabricated gold bowtie array substrates for energetics detection

An integrated field-portable surface enhanced Raman scattering (SERS) sensing system has been developed and evaluated for quantitative analysis of energetics such as perchlorate (ClO(4)(-)) and trinitrotoluene (TNT) at environmentally relevant concentrations and conditions. The detection system consists of a portable Raman spectrometer equipped with an optical fiber probe that is coupled with novel elevated gold bowtie nanostructural arrays as a sensitive and reproducible SERS substrate. Using the standard addition technique, we show that ClO(4)(-) and TNT can be quantified at concentrations as low as 0.66 mg L(-1) (or ~6.6 μM) and 0.20 mg L(-1) (~0.9 μM), respectively, in groundwater samples collected from selected military sites. This research represents the first step toward the development of a field SERS sensor which may permit rapid, in situ screening and analysis for various applications including national security, chemical, biological and environmental detection.     

Homo- and heteropolynuclear Ni2+ and Cu2+ complexes of polytopic ligands, consisting of a tren unit substituted with three 12-membered tetraazamacrocycles

Two new polytopic ligands L1 and L2 have been synthesized. They consist of a central tren unit to which three 1,4,7,10-tetraazacyclododecane rings are attached via an ethylene and a trimethylene bridge, respectively. The complexation properties of L1 and L2 towards Cu(2+) and Ni(2+) were studied by potentiometric pH titration, UV-Vis, EPR spectroscopy and kinetic techniques. As a comparison, the Cu(2+) and Ni(2+) complexes with L3 (1-(N-methyl-2-aminoethyl-1,4,7,10-tetraazacyclododecane)) were also investigated. The crystal structures of [CuL3H(H(2)O)](ClO(4))(3) and [NiL3Cl](ClO(4)) were solved and show that the side chain in its protonated form is not involved in coordination, whereas deprotonated it binds to the metal ion. The thermodynamically stable 3:1 complexes of L1 or L2 have a metal ion in the three macrocyclic units. However, when three equivalents of Cu(2+) are added to L1 or L2 the metal ion first binds to the tren unit and only then to the macrocycles. The kinetics of the different steps of complexation have been studied and a mechanism is proposed.     

Label-free, non-derivatization CRET detection platform for 6-mercaptopurine based on the distance-dependent optical properties of gold nanoparticles

A label-free, non-derivatization chemiluminescence resonance energy transfer (CRET) detection platform has been developed for the detection of the non-fluorescent small molecule 6-mercaptopurine. This CRET process arose from a chemiluminescent (CL) donor-acceptor system in which the reaction of bis(2,4,6-trichlorophenyl)oxalate (TCPO)-H(2)O(2)-fluorescein (maximum emission at 521.6 nm) served as the donor and gold nanoparticles (AuNPs, maximum absorption at 520.0 nm) served as the acceptor. This process caused a significant decrease in the CL signal of the TCPO-H(2)O(2)-fluorescein reaction. The presence of 6-mercaptopurine induced an aggregation of AuNPs with the assistance of Cu(2+) ions through cooperative metal-ligand interactions that was accompanied by a distinct change in color and optical properties. The maximum absorption band of the AuNPs was red-shifted to 721.0 nm and no longer overlapped with the CL spectrum of the reaction; as a result, the CL signal was restored. This CRET system exhibited a wide linear range, from 9.0 nmol L(-1) to 18.0 μmol L(-1), and a low detection limit (0.62 nmol L(-1)) for 6-mercaptopurine. The applicability of the proposed CRET system was evaluated by analysis of 6-mercaptopurine in spiked human plasma samples.     

Probing solution behaviour of metallosupramolecular complexes using pyrene fluorescence

A new method for assessing the topology of metallosupramolecular assemblies using pyrene-appended ligands is reported. Two potentially tetradentate ligands containing one (L(1)) and two (L(2)) terminal pyrene moieties were synthesised and their complexes with Cu(+) and Cd(2+) were characterised. Photophysical measurements demonstrate that in [Cu(2)(L(1))(2)](2+), [CdL(1)](2+) and [Cu(2)(L(2))(2)](2+) the emission spectra are dominated by monomeric emission but in the cadmium complex of L(2) (where the pyrene units are in close proximity) a quenching of the luminescence coupled with weak emission at 540 nm is indicative of excimer formation.     

Dicyanostilbene-derived two-photon fluorescence probe for free zinc ions in live cells and tissues with a large two-photon action cross section

A novel two-photon fluorescence probe for Zn(2+) derived from dicyanostilbene as a two-photon fluorophore and 4-(pyridine-2-ylmethyl)piperazine as a novel Zn(2+) ligand was developed. The probe shows a 72.5-fold fluorescence enhancement in response to Zn(2+), a large two-photon action cross-section (580 GM), a noncytotoxic effect, and pH insensitivity in the biologically relevant range, and its dissociation constant (K(d)(TP)) is 0.52 ± 0.01 μM. The probe can selectively detect free Zn(2+) ions in live cells for 1500 s or so and in living tissues at a depth of 80-150 μm without interference from other metal ions and the membrane-bound probes.     

Two-photon excited fluorescent chemosensor for homogeneous determination of copper(II) in aqueous media and complicated biological matrix

In the present work, a two-photon excited fluorescent chemosensor for Cu(2+) was prepared. The probe was constructed on the basis of internal charge transfer (ICT) principle with macrocyclic dioxotetraamine as the Cu(2+) receptor. The good water-solubility of the molecule enabled recognition and assay of Cu(2+) ions in biological media. The photophysical properties of the chemosensor were investigated in detail, exhibiting favorable fluorescence quantum yield and moderate two-photon absorption cross-section. The studies on binding thermodynamics demonstrated the formation of 1?:?1 complex between the chemosensor and Cu(2+) and an association constant of ca. 1.04 × 10(5) M(-1). Due to the rational design of the molecular structure, the sensor was highly specific to Cu(2+), which ensured high selectivity in Cu(2+) determination. Upon Cu(2+) binding, the intramolecular charge-transfer extent within the chromophore was weakened resulting in a remarkable quenching of fluorescence, based on which quantitative determination of Cu(2+) was performed. Good linearity was obtained between the fluorescence quenching value and Cu(2+) concentration ranging from 0.04 to 2.0 μM in aqueous solution. Benefiting from the merits of two-photon excitation, the chemosensor was free of interference from background luminescence in serum. A homogeneous quantitative determination of Cu(2+) was achieved in the serum medium with a linear range of 0.04 to 2.0 μM. Considering the structural flexibility of the sensor, this work also opens up the possibility to construct other two-photon excited chemosensors for direct homogeneous assay of various molecules/ions in complicated biological sample matrices.