Selective fluorometry of cytochrome c using glutathione-capped CdTe quantum dots in weakly basic medium

Glutathione-capped CdTe quantum dots (GSH-CdTe QDs) were synthesized in aqueous medium. Their interactions with proteins, especially three heme-containing proteins, were investigated over a broad pH range. At 6.0?<?pH?<?8.0, the fluorescence of the GSH-CdTe QDs can be effectively quenched by cytochrome c (Cyt. c) and hemoglobin, respectively. At pH?>?8.0, only cytochrome c quenched the fluorescence of the GSH-CdTe QDs, and no significant fluorescence changes were observed for hemoglobin or other proteins. Based on the distinct fluorescence response, a novel method has been developed for the selective determination of cytochrome c using GSH-CdTe QDs as the fluorescence probe at pH 9.0. Under optimum conditions, the linear range of the calibration curve is from 3.2?×?10^?8 to 2.4?×?10^?6?mol L^?1 and the detection limit is 3.0?×?10^?9?mol L^?1. The method has been applied to the determination of cytochrome c in three synthetic and real samples, and satisfactory results were obtained with QDs through selecting the proper pH value.     

Special characteristics of fluorescence and resonance Rayleigh scattering for cadmium telluride nanocrystal aqueous solution and its interactions with aminoglycoside antibiotics

CdTe nanocrystals (CdTe NCs) were achieved by reaction of CdCl₂ with KHTe solution and were capped with sodium mercaptoacetate. The product was detected by transmission electron microscopy (TEM), high-resolution transmission electron microscopy (HRTEM), energy dispersive spectroscopy (EDS), fluorescence spectra, ultraviolet-visible spectra and X-ray diffraction (XRD). The CdTe NCs are of cubic structure and the average size is about 5 nm. The fluorescence quantum yield of CdTe NCs aqueous solution increased from 37% to 97% after 20 d under room light. The maximum λ _em of fluorescence changed from 543 nm to 510 nm and the blue shift was 33 nm. CdTe NCs aqueous solution can be steady for at least 10 months at 4 in° a refrigerator. The resonance Rayleigh scattering (RRS) of CdTe NCs in the aqueous solution was investigated. The maximum scattering peak was located at about 554 nm. The interactions of CdTe NCs with amikacin sulfate (AS) and micronomicin sulfate (MS) were investigated respectively. The effects of AS and MS on fluorescence and RRS of CdTe NCs were analyzed. It was found that AS and MS quenched the photoluminescence of CdTe NCs and enhanced RRS of CdTe NCs. Under optimum conditions, there are linear relationships between quenching intensity (F ₀-F), intensity of RRS (I-I ₀) and concentration of AS and MS. The detection limits (3б) of AS and MS are respectively 3.4 ng·mL⁻¹ and 2.6 ng·mL⁻¹ by the fluorescence quenching method, and 15.2 ng·mL⁻¹ and 14.0 ng·mL⁻¹ by the RRS method. The methods have high sensitivity, thus CdTe NCs may be used as fluorescence probes and RRS probes for the detection of aminoglycoside antibiotics. Supported by the National Natural Science Foundation of China (Grant No. 20475045)     

Preparation and Optical Properties of CdTe/CdO-nH2O Core/shell Nano-composites in Aqueous Solution

"The deposition of CdO?nH2O on CdTe nanoparticles was studied in an aqueous phase. The CdTe nanocrystals (NCs) were prepared in aqueous solution through the reaction between Cd2+ and NaHTe in the presence of thioglycolic acid as a stabilizer. The molar ratio of the Cd2+ to Te2- in the precursory solution played an important role in the photoluminescence of the ultimate CdTe NCs. The strongest photoluminescence was obtained under 4.0 of Cd2+/Te2- at pH?8.2. With the optimum dosage of Cd(II) hydrous oxide deposited on the CdTe NCs, the photoluminescence was enhanced greatly. The photoluminescence of these nanocomposites was kept constant in the pH range of 8.0-10.0, but dramatically decreased with an obvious blue-shifted peak while the pH was below 8.0. In addition, the photochemical oxidation of CdTe NCs with cadmium hydrous oxide deposition was markedly inhibited."     

Development of a Small Molecule Probe Capable of Discriminating Cysteine,Homocysteine, and Glutathione with Three Distinct Turn‐On Fluorescent Outputs

The simultaneous discrimination of Cys, Hcy, and GSH by a single probe is still an unmet challenge. The design and synthesis of a small molecule probe MeO‐BODIPY‐Cl (BODIPY=boron dipyrromethene) is presented, which can allow Cys, Hcy, and GSH to be simultaneously discriminated on the basis of three distinct fluorescence turn‐on responses. The probe reacts with these thiols to form sulfenyl‐substituted BODIPY, which is followed by intramolecular displacement to yield amino‐substituted BODIPY. The kinetic rate of the intramolecular displacement reaction determines the observed different sensing behavior. Therefore, the probe responds to Cys, Hcy, and GSH with fluorescence turn‐on colors of yellow, yellow and red, and red, respectively. With this promising feature in hand, the probe was successfully used in imaging of Cys, Hcy and GSH in living cells.     

A dual-modal probe for NIR fluorogenic and ratiometric photoacoustic imaging of Cys/Hcy in vivo

Biothiols, such as cysteine(Cys) and homocysteine(Hcy), play vital roles in biological homeostasis and are closely related to various pathological and physiological processes in the living systems. Therefore, the in vivo detection of biothiols is of great importance for early diagnosis of diseases and assessment of disease progression. In this work, we developed a near-infrared(NIR) fluorescence and photoacoustic dual-modal molecular probe(NIR-S) that can be specifically activated by Cys or Hcy. The aryl-thioether substituted cyanine probe can undergo nucleophilic substitution and Smiles rearrangement reaction, resulting in specific turn-on NIR fluorescence and ratiometric photoacoustic responses for Hcy/Cys. Thus, NIR-S not only realizes the specific NIR fluorescence and photoacoustic dual mode imaging to detect Hcy/Cys in solution, but also can be applied to living cells and mice to detect Hcy/Cys. This work provided a practical tool to detect Hcy/Cys levels in vivo, which would be beneficial for the early diagnosis and progress of diseases.     

A colorimetric,ratiometric and water-soluble fluorescent probe for simultaneously sensing glutathione and cysteine/homocysteine

A chlorinated coumarin-aldehyde was developed as a colorimetric and ratiometric fluorescent probe for distinguishing glutathione (GSH), cystenine (Cys) and homocysteine (Hcy). The GSH-induced substitution-cyclization and Cys/Hcy-induced substitution-rearrangement cascades lead to the corresponding thiol-coumarin-iminium cation and amino-coumarin-aldehyde with distinct photophysical properties. The probe can be used to simultaneously detect GSH and Cys/Hcy by visual determination based on distinct different colors – red and pale-yellow in PBS buffer solution by two reaction sites. From the linear relationship of fluorescence intensity and biothiols concentrations, it was determined that the limits of detection for GSH, Hcy and Cys are 0.08, 0.09 and 0.18 μM, respectively. Furthermore, the probe was successfully used in living cell imaging with low cell toxicity.     

A new determining method of copper(<Emphasis Type="Bold">II</Emphasis>) ions at ng ml<Superscript>−1</Superscript> levels based on quenching of the water-soluble nanocrystals fluorescence

CdTe nanocrystals (NCs) were prepared and modified in aqueous solution by using 3-mercaptopropionic acid (MPA). Compared with previous fluorescent sensors based on organic fluorophores, these NCs have the following merits. First, they are sensitive and the synthetic procedure is simple; second, they have narrow, tunable, symmetric emission spectra and are photochemically stable. The applicability of these NCs to the determination of Cu(II) ions was studied successfully. Maximum fluorescence intensity was produced at pH 7.8, with excitation and emission wavelengths at 365 and 532 nm, respectively. Under optimal conditions, linear relationships were found between the relative fluorescence intensity and the concentration of Cu(II) ions in the range 0–256 ng ml^–1 and the limit of detection was 0.19 ng ml^–1. This method was applied to determine real samples successfully. In addition, the quenching mechanism is also described.     

Discriminatory Detection of Cysteine and Homocysteine Based on Dialdehyde‐Functionalized Aggregation‐Induced Emission Fluorophores

We demonstrate a concept‐proof work of using fluorescence (FL) “turn‐on” probes for the discriminatory detection of cysteine (Cys) over homocysteine (Hcy). The fluorogens are provided with aggregation‐induced emission (AIE) characteristic and functionalized with two aldehyde‐groups (DMTPS‐ALD and TPE‐ALD). All the detections were carried out in a biocompatible medium (10 mM HEPES buffer and DMSO, pH 7.4). In principle, the formation of thiazinane/thiazolidine through the chemical reaction of aldehydes on the probe molecules and the residue of Cys/Hcy determines the selective recognition of Cys and Hcy over other amino acids and glucose. The FL responses originate from the AIE property of thiazinane/thiazolidine resultants, which have low solubility and precipitate (aggregate) in the detection medium. The discrimination between Cys and Hcy comes from the difference in reaction kinetics of TPE‐ALD/DMTPS‐ALD with Cys and Hcy, thereby the FL responses show different time courses and intensity enhancement. It is worth noting that TPE‐ALD outshined the other two probes in performance with fast response, a high FL enhancement up to 16‐fold, high sensitivity, and good specificity and selectivity. Moreover, its FL response threshold at 250 μM is very close to the lower limit of the normal level of Cys in human plasma, which implies that TPE‐ALD could be applied as a potential indicator of Cys deficiency.     

Synthesis of Aqueous CdTe Nanocrystals with High Efficient Blue‐Green Emission of Exciton

As one of the most popular nanocrystals (NCs), aqueous CdTe NCs have very weak green emission under conventional synthesis conditions. In this work, we report the first example of blue‐emitting CdTe NCs directly synthesized in aqueous solution by slowing down the growth rate after nucleation. The key for the synthesis is the optimization of NC growth conditions, namely pH range of 7.5 to 8.5, TGA/Cd ratio of 3.6, Cd/Te ratio of 10, and Te concentration of 2×10^?5 mol/L, to get a slow growth rate after nucleation. The as‐prepared blue‐emitting CdTe NCs have small size (as small as 1.9 nm) and bright emission [with 4% photoluminescence quantum yield (PL QY) at 486 nm and 17% PLQY at 500 nm]. Transmission electron microscopy (TEM) images of the as‐prepared CdTe show monodispersed NCs which exhibit cubic zinc blend structure. Moreover, time‐resolved PL decay and X‐ray photoelectron spectroscopy (XPS) results show the as‐prepared NCs have better surface modification by ligand, which makes these luminescent small CdTe NCs have higher photoluminescence quantum yield, compared with NCs synthesized under conventional conditions.     

Preparation of monodisperse CdTe nanocrystals-SiO2 microspheres without ligands exchange

Fluorescent CdTe-SiO₂ composite microspheres were prepared by a sol–gel method without the exchange of surface ligands for the first time. We loaded CdTe nanocrystals (NCs) into the matrix of silica microspheres during the formation of composite spheres. In contrast to CdTe NCs in aqueous solutions, CdTe NCs in the composite microspheres revealed better stability while their fluorescence properties were retained due to the confined effects of silica matrix. In addition, we also investigated the dependency of properties of these composite spheres on such important synthesis factors as pH value, concentration and stabilizers during experiment procedure in details.     

CdTe nanocrystals sensitized chemiluminescence and the analytical application

It was found that the mixing of CdTe semiconductor nanocrystals (NCs) with luminol in the presence of KMnO₄ can induce a great sensitized effect on chemiluminescence (CL) emission. When the concentration of luminol, KMnO₄ and NaOH were fixed at 1 μM, 1 μM and 0.05 M, respectively, the most excellent performance can be obtained for the CdTe NCs sensitized CL. By means of CL and photoluminescence spectra, we suppose the enhanced CL signals resulted from the accelerated luminol CL induced by the oxidized species of CdTe NCs. Based on the finding, using thioglycolic acid-capped CdTe NCs as label and immunoglobulin G (IgG) as a model analyte, a CL immunoassay protocol for IgG content detection was developed. The strong inhibition effect of phenol compounds on luminol-KMnO₄-CdTe NCs CL system was also observed. All these findings demonstrated the possibility of semiconductor nanocrystals induced chemiluminescence to be utilized for more practical applications.     

Metal‐Enhanced Fluorescence of CdTe Nanocrystals in Aqueous Solution

Metal‐enhanced fluorescence of semiconductor nanocrystals (NCs) is investigated. There is very little attention paid to the metal‐enhanced fluorescence in aqueous solution, which has great potential applications in bioscience. In this work, we directly observe metal‐enhanced fluorescence of CdTe NC solution by simply mixing CdTe NCs and Au nanoparticles, both of which are negatively charged. In order to study this kind of photoluminescence enhancement in aqueous solutions, we propose a calibration method, which takes into account the light attenuation in solutions. After consideration of the light weakening in transmission, the maximal PL enhancement is about 3 times as large as the ones without Au NPs. Some factors related to the enhanced magnitude of fluorescence, for instance, the concentration and the molar feed ratio of CdTe NCs and Au NPs, are studied in detail. Furthermore, the decreased lifetimes of CdTe NCs induced by Au NPs are also obtained, which are in accord with the enhancement of the photoluminescence.     

A fluorescence turn-on probe for cysteine and homocysteine based on thiol-triggered benzothiazolidine ring formation

We synthesized a new coumarin-based probe TP, containing a disulfide moiety, to detect biothiols in cells. A fluorescence turn-on response is induced by the thiol–disulfide exchange of the probe, with subsequent intramolecular benzothiazolidine ring formation giving rise to a fluorescent product. The probe exhibits an excellent selectivity for cysteine (Cys) and homocysteine (Hcy) over glutathione (GSH) and other amino acids. The fluorescent probe also exhibits a highly sensitive fluorescence turn-on response to Cys and Hcy with detection limits of 0.8 μM for Cys and 0.5 μM for Hcy. In addition, confocal fluorescence microscopy imaging using RAW264.7 macrophages demonstrates that the probe TP could be an efficient fluorescent detector for thiols in living cells.     

α-Acrylaldehyde 3-Pyrrolyl BODIPY as a Specific Optical Sensor for Cysteine and Homocysteine

A new fluorophore, α-acrylaldehyde 3-pyrrolyl BODIPY was synthesized by treating 3-pyrrolyl BODIPY with a mixture of 3-(dimethylamino) acrolein and POCl₃ under Vilsmeier–Haack reaction conditions. The X-ray structure revealed that the fluorophore was almost planar, and the appended pyrrole was in the same plane with a small deviation from the mean plane. We investigated the potential use of α-acrylaldehyde 3-pyrrolyl BODIPY for sensing thiol containing amino acids such as cysteine/homocysteine (Cys/Hcy). Our studies showed that the α-acrylaldehyde- 3-pyrrolyl BODIPY was found to be useful for exclusive sensing of Cys/Hcy and to exhibit different optical signaling responses to Cys and Hcy at physiological pH in aq. CH₃CN (1 : 1 v/v, PBS) medium. The enhancement in optical properties for Cys and quenching in same properties for Hcy was attributed to different binding modes of Cys/Hcy with α-acrylaldehyde 3-pyrrolyl BODIPY.     

A multisite-binding fluorescent probe for simultaneous monitoring of mitochondrial homocysteine,cysteine and glutathione in live cells and zebrafish

Homocysteine(Hcy), cysteine(Cys) and glutathione(GSH) play crucial roles in redox homeostasis during mitochondria functions. Simultaneous differentiation and visualization of mitochondrial biothiols dynamics are significant for understanding cell metabolism and their related diseases. Herein, a multisitebinding fluorescent probe(MCP) was developed for simultaneous sensing of mitochondrial Cys, GSH and Hcy from three fluorescence channels for the first time. This novel probe exhibited rapid fluor...     

Dual‐Emission Channels for Simultaneous Sensing of Cysteine and Homocysteine in Living Cells

The development of a fluorescent probe to distinguish between cysteine (Cys) and homocysteine (Hcy) is always a challenge owing to their structural similarity, and the simultaneous detection of Cys and Hcy by utilizing different emission channels is especially difficult. In this work, we designed and synthesized a new fluorescent probe to differentiate between Cys and Hcy on the basis of a coumarin derivative with a chlorine atom and an α,β‐unsaturated aldehyde. Cys and Hcy induced different cascade reactions with the probe, which led to different products with distinct photophysical properties. The nonfluorescent probe responded to Cys and emitted strong blue fluorescence, whereas it reacted with Hcy and generated yellow fluorescence without interference from glutathione. In addition, the probe was successfully applied to distinguish between Cys and Hcy in living cells.     

Facile synthesis of nanocrystal encoded fluorescent silica microspheres

Monodisperse CdTe composite microspheres with a spherical shape were prepared using organosilane chemicals in aqueous solution. CdTe nanocrystals (NCs) were loaded into the matrix of silica microspheres during the formation of composite microspheres. Detailed characterization of the CdTe composite microspheres by scanning electron microscopy (SEM), transmission electron microscopy (TEM), and spectrofluorimeter was performed to elucidate the morphology and fluorescence of the composite microspheres. In contrast to CdTe NCs in aqueous solution, CdTe NCs in the composite microspheres revealed high stability and fluorescence due to the confined effects of silica matrix. In addition, multicolored CdTe QDs were encoded into the microspheres at precise ratios.     

Rational Design of an “OFF–ON” Phosphorescent Chemodosimeter Based on an Iridium(III) Complex and Its Application for Time‐Resolved Luminescent Detection and Bioimaging of Cysteine and Homocysteine

Biothiols, such as cysteine (Cys) and homocysteine (Hcy), play very crucial roles in biological systems. Abnormal levels of these biothiols are often associated with many types of diseases. Therefore, the detection of Cys (or Hcy) is of great importance. In this work, we have synthesized an excellent “OFF‐ON” phosphorescent chemodosimeter 1 for sensing Cys and Hcy with high selectivity and naked‐eye detection based on an Ir^III complex containing a 2,4‐dinitrobenzenesulfonyl (DNBS) group within its ligand. The “OFF‐ON” phosphorescent response can be assigned to the electron‐transfer process from Ir^III center and C^N ligands to the DNBS group as the strong electron‐acceptor, which can quench the phosphorescence of probe 1 completely. The DNBS group can be cleaved by thiols of Cys or Hcy, and both the ³M LCT and ³LC states are responsible for the excited‐state properties of the reaction product of probe 1 and Cys (or Hcy). Thus, the phosphorescence is switched on. Based on these results, a general principle for designing “OFF‐ON” phosphorescent chemodosimeters based on heavy‐metal complexes has been provided. Importantly, utilizing the long emission‐lifetime of phosphorescence signal, the time‐resolved luminescent assay of 1 in sensing Cys was realized successfully, which can eliminate the interference from the short‐lived background fluorescence and improve the signal‐to‐noise ratio. As far as we know, this is the first report about the time‐resolved luminescent detection of biothiols. Finally, probe 1 has been used successfully for bioimaging the changes of Cys/Hcy concentration in living cells.     

A validated HPLC‐fluorescence method with a semi‐micro column for routine determination of homocysteine,cysteine and cysteamine,and the relation between the thiol derivatives in normal human plasma

A semi‐micro column HPLC‐fluorescence method for routine determination of thiol derivatives such as homocysteine (Hcy), cysteine (Cys) and cysteamine (CA) is described. The thiol derivatives labeled with ammonium‐7‐fluorobenzo‐2‐oxa‐1,3‐diazole‐4‐sulfonate (SBD‐F) were isocratically separated within 12 min on a semi‐micro ODS column (Daisopak‐SP‐120‐5‐ODS‐BP) with a mixture of 25 mm acetate buffer (pH 2.00) and CH₃CN as a mobile phase. The purity and similarity of SBD‐thiols by a multi‐wavelength fluorescence detector were more than 92.3 and 96.7%. The detection limits of Hcy, Cys and CA at a signal‐to‐noise ratio of 3 were 0.16, 0.47 and 0.03 µm , respectively. Furthermore validation parameters such as accuracy, precision and robustness of the proposed method showed satisfactory results. Almost 850 plasma sample injections (range 572–1076, n = 3) for a column could be performed without differences in retention time and peak heights of labels. As an application of the proposed method, the determination of thiol derivatives in normal human plasma (n = 103) was demonstrated. The correlation coefficients between Hcy vs Cys and Hcy vs CA were 0.38 and −0.35, respectively. Copyright © 2009 John Wiley & Sons, Ltd.     

(Yb3+, Mn2+) Co-doped CdTe nanocrystals with enhanced quantum yields and red-shift emission

We prepared the nanocrystals (NCs) of CdTe, CdTe:Yb, and CdTe:Yb, Mn vis water phase synthesis and examined their structural, morphological, and optical properties. All NCs have a particle diameter of about 2–4 nm, and the monodispersed, uniform spherical, cubic structure of the CdTe NC remains largely unchanged after the doping with Yb and Mn. According to the X-ray diffraction results, the CdTe, CdTe:Yb, and CdTe:Yb, Mn NCs all have a cubic structure, and the diffraction peak of CdTe:Yb NC is at a lower 2θ angle compared with that of the CdTe NC. With the CdTe NC as the reference, the UV–Vis absorption of the CdTe:Yb and the CdTe:Yb, Mn NCs exhibits a blueshift and a redshift, and the emission of CdTe:Yb and CdTe:Yb, Mn has a blueshift of about 12 nm and a redshift of about 73 nm, respectively. The CdTe:Yb, Mn NCs have higher quantum yields than the CdTe:Yb NC, and the quantum yield is the highest when CdTe is doped with 1:1 Mn²⁺/Yb³⁺. In addition, both the CdTe:Yb and CdTe:Yb, Mn NCs have a shorter fluorescence lifetime than the CdTe NC.