Highly Selective and Sensitive Near‐Infrared‐Fluorescent Probes for the Detection of Cellular Hydrogen Sulfide and the Imaging of H2S in Mice

Herein, we report the development of two fluorescent probes for the highly selective and sensitive detection of H₂S. The probes take advantage of a Cu^II? cyclen complex, which acts as a reaction center for H₂S and as a quencher of BODIPY (boron‐dipyrromethene)‐based fluorophores with emissions at 765 and 680 nm, respectively. These non‐fluorescent probes could only be turned on by the addition of H₂S, and not by other potentially interfering biomolecules, including reactive oxygen species, cysteine, and glutathione. In a chemical system, both probes detected H₂S with a detection limit of 80 nM . The probes were successfully used for the endogenous detection of H₂S in HEK 293 cells, for measuring the H₂S‐release activity of dietary organosulfides in MCF‐7 cells, and for the in vivo imaging of H₂S in mice.     

Small-molecule fluorescent probes for imaging gaseous signaling molecules: current progress and future implications

Endogenous gaseous signaling molecules including nitric oxide (NO), carbon monoxide (CO) and hydrogen sulfide (H₂S) have been demonstrated to perform significant physiological and pharmacological functions and are associated with various diseases in biological systems. In order to obtain a deeper insight into their roles and mechanisms of action, it is desirable to develop novel techniques for effectively detecting gaseous signaling molecules. Small-molecule fluorescent probes have been proven to be a powerful approach for the detection and imaging of biological messengers by virtue of their non-invasiveness, high selectivity, and real-time in situ detection capability. Based on the intrinsic properties of gaseous signaling molecules, numerous fluorescent probes have been constructed to satisfy various demands. In this perspective, we summarize the recent advances in the field of fluorescent probes for the detection of NO, CO and H₂S and illustrate the design strategies and application examples of these probes. Moreover, we also emphasize the challenges and development directions of gasotransmitter-responsive fluorescent probes, hoping to provide a general implication for future research.

This perspective article aims to introduce the design principles and recognition strategies of small-molecule fluorescent probes which are applied for the detection of gas signaling molecules including NO, CO and H₂S in biological systems.     

Dual‐Reactable Fluorescent Probes for Highly Selective and Sensitive Detection of Biological H2S

Hydrogen sulfide (H₂S) is an important endogenous signaling molecule with a variety of biological functions. Development of fluorescent probes for highly selective and sensitive detection of H₂S is necessary. We show here that dual‐reactable fluorescent H₂S probes could react with higher selectivity than single‐reactable probes. One of the dual‐reactable probes gives more than 4000‐fold turn‐on response when reacting with H₂S, the largest response among fluorescent H₂S probes reported thus far. In addition, the probe could be used for high‐throughput enzymatic assays and for the detection of Cys‐induced H₂S in cells and in zebrafish. These dual‐reactable probes hold potential for highly selective and sensitive detection of H₂S in biological systems.     

Perspectives of magnetic nature carbon dots in analytical chemistry: From separation to detection and bioimaging

Magnetic nature carbon dots (MNCDs) are fast growing materials with extremely unique physico-chemical properties and physiological ability to extend their applications from separation science to detection and bio-/magnetic resonance imaging applications. Recent studies have revealed that the MNCDs are significantly used as promising agents in analytical chemistry for the separation and identification of trace level target analytes. Further, the MNCDs have been used as probes for bioimaging of cells and magnetic resonance imaging (MRI) of tumors. Due to the lack of comprehensive reviews in this emerging field especially MNCDs applications in analytical chemistry, this review may provide quick guide and reference on the MNCDs-based analytical approaches for the separation and detection of trace level analytes, and bio- and MR- imaging of various cells. In this review article, we will summarize the synthetic approaches for the fabrication of MNCDs. The main part of this proposed review is devoted to the tremendous applications of MNCDs (Fe₃O₄@CDs, metal ion (Fe³⁺, Mn²⁺, Co²⁺ and Gd²⁺)-doped CDs, MnO₂@CDs) in analytical chemistry from separation science to detection and bio- and MR imaging. Finally, we will explore the challenges and future prospects of magneto fluorescent carbon dots in biomedical applications.     

Determination Limit of Fluorescence Turn‐On Probes for the Acetate Anion

Three fluorescent turn‐on probes containing 3,6‐dichloro‐9H‐carbazole as carbazyl part have been designed and synthesized. Among studied anions F^?, AcO^?, H₂PO , Cl^?, Br^? and I^?, AcO^? showed the strongest binding ability with all probes. The strong basic anions, such as AcO^?, H₂PO , and F^?, induced a significant red‐shift in absorption and a concomitant increase in fluorescent emission of the probes caused by photoinduced electron transfer (PET). The determination limit of probe 3 (Scheme 1) toward AcO^? is 3.0×10^?7 M . ¹H‐NMR Titration experiments shed light on the nature of the interaction between the probes and the anions. Theoretical investigation further illustrated the possible binding mode in these host? guest interactions and the roles of molecular frontier orbitals in molecular interplay.     

Novel Fluorescent Probes for Singlet Oxygen

The first fluorescent chemical traps for ¹ O ₂ have been developed. DPAXs react specifically with ¹O₂ to yield the corresponding endoperoxides, DPAX-EPs (see scheme; X = H, Cl, F). DPAXs scarcely fluoresce, while DPAX-EPs are strongly fluorescent. Since the fluorescence of these probes is unaffected by H₂O₂, superoxide, and nitric oxide, they are useful for the selective detection of ¹O₂ in biological systems.     

Porous Molybdenum Carbide Nanostructured Catalyst toward Highly Sensitive Biomimetic Sensing of H2O2

There are great challenges to fabricate a highly selective and sensitive enzyme‐free biomimetic sensor. Herein for the first time a unique nanostructure of porous molybdenum carbide impregnated in N‐doped carbon (p‐Mo₂C/NC) is synthesized by using SiO₂ nanocrystals‐templating method and is further used as an enzyme‐free electrochemical biosensor toward highly selective, sensitive detection of H₂O₂, of which the limit of detection, dynamic detection range and sensitivity accomplish as 0.22 μM, 0.05–4.5 mM and 577.14 μA mM^?1 cm^?2, respectively, and are much superior to the non‐porous molybdenum carbide impregnated in N‐doped carbon (Mo₂C/NC). The sensor is also used to monitor H₂O₂ released from A549 living cells. This work holds a great promise to be used to monitor the presence of H₂O₂ in biological research while offering an important knowledge to design a highly selective and sensitive biomimetic sensor by synthesizing a porous catalyst to greatly improve the reaction surface area rather than conventionally only relying on dispersing the catalyst material into porous carbon substrate.     

Colorimetric and ratiometric sensors derivated from natural building blocks for fluoride ion detection

Three novel colorimetric and ratiometric probes (SH-1~3) for fluoride ion detection were designed and synthesized from nature small molecules. Obvious yellow-to-orange color change of these probes in the THF was achieved only in presence of F^? among the eight anions (F^?, Cl^?, Br^?, I^?, H₂PO₄^?, HSO₄^?, CH₃COO^–, ClO₄^?), along with the emission shifting from green to orange red. These three probes are 1:1 complexed with fluoride ions, with complexation constant of around 0.1 × 10⁴ M^?1. The detection limit of probes SH-1~3 reached as low as around 1 μM. ¹H NMR titration study suggested that the fluoride ion induced deprotonation of the probe through hydrogen bonding interaction between amino group of probe and fluoride ion.     

Recent advances in fluorescent probes for the detection of reactive oxygen species

Reactive oxygen species (ROS) have captured the interest of many researchers in the chemical, biological, and medical fields since they are thought to be associated with various pathological conditions. Fluorescent probes for the detection of ROS are promising tools with which to enhance our understanding of the physiological roles of ROS, because they provide spatial and temporal information about target biomolecules in in vivo cellular systems. ROS probes, designed to detect specific ROS with a high selectivity, would be desirable, since it is now becoming clear that each ROS has its own unique physiological activity. However, dihydro-compounds such as 2′,7′-dichlorodihydrofluorescein (DCFH), which have traditionally been used for detecting ROS, tend to react with a wide variety of ROS and are not completely photostable. Some attractive fluorescent probes that exhibit a high degree of selectivity toward specific ROS have recently been reported, and these selective probes are expected to have great potential for elucidating unknown physiological mechanisms associated with their target ROS. This review focuses on the design, detection mechanism, and performance of fluorescent probes for the detection of singlet oxygen (¹O₂), hydrogen peroxide (H₂O₂), hydroxyl radicals (^.OH), or superoxide anion (O₂ ^−.), a field in which remarkable progress has been achieved in the last few years.     

Comparison of efficiencies between single-drop microextraction and continuous-flow microextraction for the determination of methomyl in natural waters

Two liquid-phase microextraction (LPME) approaches, static direct-immersed single-drop microextraction (DI-SDME) and continuous-flow microextraction (CFME), were used to extract methomyl in water samples and their respective extraction efficiencies were compared. Several important parameters affecting extraction efficiency such as the type of extraction solvent, solvent drop volume, stirring speed or flow rate, extraction time and salt concentration were optimised. The optimised conditions were as follows: 3.0-µL tetrachloroethane (C₂H₂Cl₄) as the extraction solvent, 15% NaCl (w/v), 15 min extraction time and stirring speed at 600 rpm for DI-SDME; 3.5-µL C₂H₂Cl₄ as the extraction solvent, 15% NaCl (w/v), 21 min extraction time and flowing rate at 0.8 mL min^?1 for CFME. Under the previous optimal conditions, the linear range, detection limit (S/N = 3) and precision (RSD, n = 6) were 5.0-5000 ng mL^?1, 1.5 ng mL^?1, 6.9% for DI-SDME, and 4.0–10000 ng mL^?1, 2.5 ng mL^?1, 4.6% for CFME, respectively. Lake and river water samples were successfully analysed by DI-SDME and CFME. The result demonstrated that both SDME and CFME techniques are simple, low cost and amity to environment. As a result, the two approaches have tremendous potential in trace analysis of methomyl in natural waters.     

Graphene oxide coated capillary for the analysis of endocrine‐disrupting chemicals by open‐tubular capillary electrochromatography with amperometric detection

A graphene oxide‐coated capillary was fabricated by using 3‐aminopropyltriethoxysilane as the cross‐linking agent. It was used for the separation and detection of three endocrine‐disrupting chemicals, including bisphenol A, 4‐nonylphenol, and 4‐octylphenol by capillary electrochromatography. Due to the hydrophobicity, hydrogen bonding, and π–π interaction between graphene oxide and the analytes, the three analytes could be well separated in pH = 11.0, 20 mmol/L Na₂B₄O₇‐NaOH/methanol mobile phase (50:50, v/v) within 950 s. After preconcentration, the detection limits were 6.7 × 10^?10, 3.3 × 10^?9, and 6.7 × 10^?10 mol/L (S/N = 3) for bisphenol A, nonylphenol, and octylphenol, respectively. The developed method was successfully applied to the determination of the above analytes in water samples. The satisfactory result demonstrated that the graphene oxide coated capillary used in capillary electrochromatography with amperometric detection was convenient to prepare, highly stable, and had good reproducibility.     

Novel Fluorescent Chemosensor for Detection of F− Anions Based on a Single Functionalized Pillar[5]arene Iron(III) Complex

Novel fluorescent chemosensor with good selectivity for F^? anion was designed and synthesized. The sensor has a bearing on a single functionalized pillar[5]arene and Fe³⁺ metal complex (PN‐Fe), which showed prominent fluorescent response for F^? anion over other common anions (Cl^?, Br^?, I^?, AcO^?, HSO4^?, H₂PO₄^?, ClO₄^?, CN^? and SCN^?). These results were evaluated by fluorescent method. The detection limit of PN‐Fe to F^? was calculated to be 2.50×10^?7 mol/L. Moreover, the sensor PN‐Fe³⁺ might serve as a recyclable component in sensing materials.     

Reactivity in the gas phase. Behaviour of isoxazoles under negative ion chemical ionization conditions

[M ? H⁺]^? ions of isoxazole (la), 3-methylisoxazole (1b), 5-methylisoxazole (1c), 5-phenylisoxazole (1d) and benzoylacetonitrile (2a) are generated using NICI/OH^? or NICI/NH₂^? techniques. Their fragmentation pathways are rationalized on the basis of collision-induced dissociation and mass-analysed ion kinetic energy spectra and by deuterium labelling studies. 5-Substituted isoxazoles 1c and 1d, after selective deprotonation at position 3, mainly undergo N ? O bond cleavage to the stable α-cyanoenolate NC ? CH ? CR ? O^? (R = Me, Ph) that fragments by loss of R? CN, or R? H, or H₂O. The same α-cyanoenolate anion (R = Ph) is obtained from 2a with OH^?, or NH₂^?, confirming the structure assigned to the [M ? H⁺]^? ion of 1d, On the contrary, 1b is deprotonated mainly at position 5 leading, via N? O and C(3)? C(4) bond cleavages, to H? C ≡ C? O ^? and CH₃CN. Isoxazole (1a) undergoes deprotonation at either position and subsequent fragmentations. Deuterium labelling revealed an extensive exchange between the hydrogen atoms in the ortho position of the phenyl group and the deuterium atom in the α-cyanenolate NC ? CD = CPh ? O^?.     

Piaselenol—Piaselenolium—Pentaiodid (C6H4N2Se · C6H5N2Se+I3− · I2), eine Struktur mit Polyiodid-schichten

Piaselenole—Piaselenolium—Pentaiodide (C₆H₄N₂Se · C₆H₅N₂Se⁺ I₃^? · I₂), a Structure with Polyiodide Layers The title compound crystallizes in the monoclinic space group P2₁/n with a = 9.320(3), b = 13.812(2), c = 17.159(3) Å, β = 96.11(2)°, V = 2196.3 ų, Z = 4. There occur no isolated I^5? anions but layer-shaped polyiodide aggregates built up by linear, asymmetric I₃^? anions and I₂ molecules. Almost linear triiodide chains are connected by I₂ molecules in a novel type of arrangement to form slightly puckered layers. The polyiodide layers contain several substructures known from other examples. The piaselenole and its conjugated acid, the piaselenolium cation, form a ribbon-like quasi-polymer in which the two components are alternating. They are connected in turns by a linear NH? N hydrogen bridge (N? N: 2.844 Å) and by a so called (SeN)₂-connectivity parallelogram, in which Se? N bonds and Se? N contacts are adjacent. Here we found a very short Se? N contact distance of 2.691 Å. The bond distances of piaselenole (Se? N: 1.787(3) Å, N? C: 1.318(5) Å, C? C: 1.453(8) Å) and also the angles are equal or similar to those occuring in other 1,2,5-selenadiazoles. The protonation of one N in the SeN₂ unit results in a loss of symmetry and significant changes in bonding distances and angles.     

Sulfonate-based fluorescent probes for imaging hydrogen peroxide in living cells

Based on the mechanism of H₂O₂-mediated hydrolysis of sulfonates, two fluorescein disulfonates compounds (FS-1 and FS-2) were designed and synthesized as the highly selective and sensitive fluorescent probes for imaging H₂O₂ in living cells. The probes were detected with elemental analysis, IR, ¹H NMR and ¹³C NMR. Upon reaction with H₂O₂, the probes exhibit strong fluorescence responses and high selectivity for H₂O₂ over other reactive oxygen species and some biological compounds. Furthermore, the sulfonate-based probes, as novel fluorescent reagents, are cell-permeable and can detect micromolar changes in H₂O₂ concentrations in living cells by using confocal microscopy. Supported by the National Basic Research Program of China (Grant No. 2007CB936000), the National Natural Science Funds for Distinguished Young Scholar (Grant No. 20725518), Major Program of the National Natural Science Foundation of China (Grant No. 90713019), the National Natural Science Foundation of China (Grant No. 20875057), the Natural Science Foundation of Shandong Province, China (Grant No. Y2007B02), and the Science and Technology Development Programs of Shandong Province, China (Grant No. 2008GG30003012)     

Homo‐ and Heterodinuclear Ir and Rh Imine‐functionalized Protic NHC Complexes: Synthetic,Structural Studies,and Tautomerization/Metallotropism Insights

The influence of the potentially chelating imino group of imine‐functionalized Ir and Rh imidazole complexes on the formation of functionalized protic N‐heterocyclic carbene (pNHC) complexes by tautomerization/metallotropism sequences was investigated. Chloride abstraction in [Ir(cod)Cl{C₃H₃N₂(DippN=CMe)‐κN3}] ( 1 a ) (cod=1,5‐cyclooctadiene, Dipp=2,6‐diisopropylphenyl) with TlPF₆ gave [Ir(cod){C₃H₃N₂(DippN=CMe)‐κ²(C2,N_imine)}]⁺[PF₆]^? ( 3 a ⁺[PF₆]^?). Plausible mechanisms for the tautomerization of complex 1 a to 3 a ⁺[PF₆]^? involving C2?H bond activation either in 1 a or in [Ir(cod){C₃H₃N₂(DippN=CMe)‐κN3}₂]⁺[PF₆]^? ( 6 a ⁺[PF₆]^?) were postulated. Addition of PR₃ to complex 3 a ⁺[PF₆]^? afforded the eighteen‐valence‐electron complexes [Ir(cod)(PR₃){C₃H₃N₂(DippN=CMe)‐κ²(C2,N_imine)}]⁺[PF₆]^? ( 7 a ⁺[PF₆]^? (R=Ph) and 7 b ⁺[PF₆]^? (R=Me)). In contrast to Ir, chloride abstraction from [Rh(cod)Cl{C₃H₃N₂(DippN=CMe)‐κN3}] ( 1 b ) at room temperature afforded [Rh(cod){C₃H₃N₂(DippN=CMe)‐κN3}₂]⁺[PF₆]^? ( 6 b ⁺[PF₆]^?) and [Rh(cod){C₃H₃N₂(DippN=CMe)‐κ²(C2,N_imine)}]⁺[PF₆]^? ( 3 b ⁺[PF₆]^?) (minor); the reaction yielded exclusively the latter product in toluene at 110 °C. Double metallation of the azole ring (at both the C2 and the N3 atom) was also achieved: [Ir₂(cod)₂Cl{μ‐C₃H₂N₂(DippN=CMe)‐κ²(C2,N_imine),κN3}] ( 10 ) and the heterodinuclear complex [IrRh(cod)₂Cl{μ‐C₃H₂N₂(DippN=CMe)‐κ²(C2,N_imine),κN3}] ( 12 ) were fully characterized. The structures of complexes 1 b , 3 b ⁺[PF₆]^?, 6 a ⁺[PF₆]^?, 7 a ⁺[PF₆]^?, [Ir(cod){C₃HN₂(DippN=CMe)(DippN=CH)(Me)‐κ²(N3,N_imine)}]⁺[PF₆]^? ( 9 ⁺[PF₆]^?), 10? Et₂O ? toluene, [Ir₂(CO)₄Cl{μ‐C₃H₂N₂(DippN=CMe)‐κ²(C2,N_imine),κN3}] ( 11 ), and 12? 2 THF were determined by X‐ray diffraction.     

Less Is More: Three‐Coordinate C,N‐Chelated Distannynes and Digermynes

We report here the synthesis of new C,N‐chelated chlorostannylenes and germylenes L³MCl (M=Sn( 1 ), Ge ( 2 )) and L⁴MCl (M=Sn( 3 ), Ge ( 4 )) containing sterically demanding C,N‐chelating ligands L^{3, 4} (L³=[2,4‐di‐tBu‐6‐(Et₂NCH₂)C₆H₂]^?_; L⁴=[2,4‐di‐tBu‐6‐{(C₆H₃‐2′,6′‐iPr₂)N=CH}C₆H₂]^?). Reductions of 1 – 4 yielded three‐coordinate C,N‐chelated distannynes and digermynes [L^{3, 4}M ]₂ for the first time ( 5 : L³, M=Sn, 6 : L³, M=Ge, 7 : L⁴, M=Sn, 8 : L⁴, M=Ge). For comparison, the four‐coordinate distannyne [L⁵Sn]₂ ( 10 ) stabilized by N,C,N‐chelate L⁵ (L⁵=[2,6‐{(C₆H₃‐2′,6′‐Me₂)N?CH}₂C₆H₃]^?) was prepared by the reduction of chlorostannylene L⁵SnCl ( 9 ). Hence, we highlight the role of donor‐driven stabilization of tetrynes. Compounds 1 – 10 were characterized by means of elemental analysis, NMR spectroscopy, and in the case of 1 , 2 , 5 – 7 , and 10 , also by single‐crystal X‐ray diffraction analysis. The bonding situation in either three‐ or four‐coordinate distannynes 5 , 7 , and 10 was evaluated by DFT calculations. DFT calculations were also used to compare the nature of the metal–metal bond in three‐coordinate C,N‐chelating distannyne [L³Sn]₂ ( 5 ) and related digermyme [L³Ge]₂ ( 6 ).     

STUDIES ON THE BACTERIAL ACTIVITY OF COBALT(III) COMPLEXES. PART III. COBALT(III) CARBOXYLATE COMPLEXES

Abstract

Cobalt(III) complexes of the type [Co(en)₂(chel)]X.nH₂O where en = ethylenediamine, chel = phthalato = C₆H₄CO₂)^2? ₂, maleato = (O₂CCH = CHCO₂)^2?, succinato = (O₂CCH₂CH₂CO₂)^2?, homophthalato = (O₂CC₆H₄(CH₂)CO₂)^2?, citraconato = (O₂CC(CH₃) = CHCO₂)^2?, itaconato = (CH₂ = C(CO₂)CH₂CO₂)^2?, X = NO^? ₃, Br^?, (O₂CC₆H₄CO₂H)^?, (O₂CHC = CHCO₂H)^?, (O₂C(CH₂)₂CO₂H)^?, (O₂CC₆H₄(CH₂)CO₂H)^?, (O₂CHC = C(CH₂)-CO₂H)^?, and (O₂C-CH₂?C(= CH₂)-CO₂H)^?, [Co(en)₂(malonato)]X.2H₂O (where malonato = (O₂CCH₂CO₂)^2?, X = Cl^?, Br^?, and NO^? ₃) and [Co(en)₂CO₃]Cl.2H₂O have been investigated for their bacterial activity against Escherichia coli B growing on EMB agar and in minimal glucose media both in lag and log phases. Among the most active are where chel = phthalato and homophthalato. The effects are distinct from those known for compounds of Pt, e.g., cis?[Pt(NH₃)₂Cl₂] and rhodium, e.g., trans?[Rh(C₅H₅N)₄,Cl₂].6H₂O. Antagonisms are reported.     

Fluorogenic Probe Using a Mislow–Evans Rearrangement for Real-Time Imaging of Hydrogen Peroxide

Hydrogen peroxide (H₂O₂) mediates the biology of wound healing, apoptosis, inflammation, etc. H₂O₂ has been fluorometrically imaged with protein- or small-molecule-based probes. However, only protein-based probes have afforded temporal insights within seconds. Small-molecule-based electrophilic probes for H₂O₂ require many minutes for a sufficient response in biological systems. Here, we report a fluorogenic probe that selectively undergoes a [2,3]-sigmatropic rearrangement (seleno-Mislow-Evans rearrangement) with H₂O₂, followed by acetal hydrolysis, to produce a green fluorescent molecule in seconds. Unlike other electrophilic probes, the current probe acts as a nucleophile. The fast kinetics enabled real-time imaging of H₂O₂ produced in endothelial cells in 8 seconds (much earlier than previously shown) and H₂O₂ in a zebrafish wound healing model. This work may provide a platform for endogenous H₂O₂ detection in real time with chemical probes.     

Spectrophotometric determination of oxyhalides with N,N-diethylaniline

We have developed procedures for the spectrophotometric determination of ClO^?, BrO ₃ ^? , and IO ₃ ^? in waters of different origin. The procedures are based on the oxidation of N,N-diethylaniline in acidic media and their detection limits (by 3s criterion) are 0.04, 0.18, and 0.53 ??g/mL, respectively. The calibration curves are linear in the concentration ranges 0.1?C2.0, 0.4?C12.5, and 1.6?C40 ??g/mL, respectively. The procedures provide simple and rapid determination of these analytes.