New validated HPLC methodology for the determination of (−)-trans-paroxetine and its enantiomer in pharmaceutical formulations with use of ovomucoid chiral stationary phase

A new chromatographic method for the enantioseparation and the determination of (?)-trans-paroxetine and (+)-trans-paroxetine has been developed with the aid of amylose ovomucoid-based chiral stationary phase. The method is faster and five times more sensitive than procedures recommended previously: limit of detection and limit of quantification are 5 and 16 ng/mL, respectively [modified (Ferretti et al. in J Chromatogr B 710:157–164, 1998): 20 and 60 ng/mL]. It was carefully validated and applied for the determination of (?)-trans-paroxetine and (+)-trans-paroxetine in Parogen (Mc Dermott Laboratories Ltd.) and Xetanor (Actavis) coated tablets.

A novel anti-interference and pH-modulation device: application to enzyme-free glucose detection

We report on a novel anti-interference and pH-modulation device (herein after referred to as ??device??). It is based on electrodialysis and can continuously increase the pH value of the carrier solution and - at the same time - remove interfering analytical signals obtained for ascorbic acid (AA) and uric acid (UA). The ??device?? was coupled to the FIA-amperometric detection of glucose. The linear range is from 1???mol?L^?1 to 0.4?mmol?L^?1, with a sensitivity of 213???A?cm^?2?mM^?1 and a detection limit of 1???mol?L^?1 at a signal-to-noise ratio of 3. The method was used to sucessfully determine glucose in serum. This study represents a novel technique for overcoming analytical interference and is expected to find applications in liquid chromatography, for example in on-line pH-modulation if different pH values are needed for separation and detection.

New disaccharide blocks for OSW-1 and its analogs

A new disaccharide block for OSW-1 natural steroidal antitumor agent was described. Regioisomeric 2- and 3-O-p-methoxybenzoyl derivatives of phenyl 1-thio-??-d-xylopyranoside and phenyl 2-O-acetyl-1-thio-??-l-arabinopyranoside derivatives blocked at positions 3 and 4 by R₃Si groups were synthesized with a view to use them in the preparation of OSW-1 analogs modified at the disaccharide fragment.     

Synthesis and crystal structure of the complex N,N-dimethylanilinium dicitratoborate monohydrate

N,N-Dimethylanilinium dicitratoborate monohydrate [C₆H₅NH(CH₃)₂][(C₆H₆O₇)₂B]·H₂O (I) was synthesized for the first time. Single crystals were obtained in an aqueous solution; the crystal structure was studied by X-ray crystallography. Crystals of I are triclinic, space group $P\bar 1$ , a = 9.7017(2) ?, b = 11.0475(2) ?, c = 12.6282(2) ?, ?? = 106.595(2)°, ?? = 106.931(1)°, ?? = 103.568(1)°, V = 1163.97(4) ?³, Z = 2, ??_calc = 1.516 g/cm³. The structural units of compound 1 are large complex dicitratoborate anions with a spiran structure, N,N-dimethylanilinium cations, and crystal water molecules. The crystal packing is a three-dimensional framework. A hydrogen-bond system is formed by seven independent contacts O(N)-H??O.     

Synthesis, crystal structures, DNA binding and cleavage studies of two oxovanadium(IV) complexes of 1,10-phenanthroline and Schiff bases derived from tryptophan

Two new V(IV) complexes, [VO(Naph?Ctrp)(phen)]·CH₃OH (1) and [VO(o-Van?Ctrp)(phen)]·CH₃OH·H₂O (2) (Naph?CTrp?=?Schiff base derived from 2-hydroxy-1-naphthaldehyde and l-tryptophan, o-Van?Ctrp?=?Schiff base derived from o-vanillin and l-tryptophan, phen?=?1,10-phenanthroline), have been synthesized and characterized by physicochemical methods. The V(IV) atoms in both complexes are six-coordinated in a distorted octahedral environment. In the crystals of complex 1, the C?CH···?? and ?ШC?? stacking interactions form a 1D chain structure, whereas for complex 2, hydrogen bonds connect the molecular units into a 2D plane structure. The DNA binding properties and cleavage efficiencies of the complexes have been investigated by spectroscopic methods, viscosity measurements and agarose gel electrophoresis. The results suggest that both complexes can bind to CT-DNA in an intercalative mode and can also cleave pBR322 DNA.     

Magnetic properties and BSA adsorption of nano-Fe-embedded BaFe12O19 porous microfibers via organic gel-thermal selective reduction process

Magnetic nano-Fe-embedded BaFe₁₂O₁₉ (NFEB) porous microfibers with diameters about 1?C5???m were prepared by the organic gel-thermal selective reduction process. The NFEB porous microfibers were formed after reduction of the precursor Fe₂O₃?CBaFe₁₂O₁₉ microfibers at 350?°C for 1?h. The precursor Fe₂O₃?CBaFe₁₂O₁₉ microfibers were obtained by calcination of the gel fibers. In the NFEB porous microfibers, the cubic ??-Fe particles with size about 300?nm are homogeneously embedded in the hexagonal plate-like barium ferrite and the pore sizes are around 50?C150?nm. The magnetic properties of these NFEB porous microfibers are influenced by the mass ratio of ??-Fe/BaFe₁₂O₁₉ and reduction conditions. The NFEB porous microfibers with the designed soft (??-Fe)/hard (BaFe₁₂O₁₉) mass ratio of 1/2 obtained at 375?°C for 1?h have the enhanced saturation magnetization (M _sh ) of 73.9?Am²?kg^?1, coercivity (H _c ) of 81.6?kAm^?1 and remanence (M _r ) of 34.2?Am²?kg^?1, compared to the single phase of BaFe₁₂O₁₉ and ??-Fe microfibers. This enhanced magnetic properties can be attributed to the exchange-coupling interactions. The NFEB porous microfibers exhibit a higher BSA adsorption capability than each single phase of ??-Fe microfibers and BaFe₁₂O₁₉ microfibers. The BSA adsorption is analyzed.     

Soft Ionization of Saturated Hydrocarbons, Alcohols and Nonpolar Compounds by Negative-Ion Direct Analysis in Real-Time Mass Spectrometry

Large polarizable n-alkanes (approximately C18 and larger), alcohols, and other nonpolar compounds can be detected as negative ions when sample solutions are injected directly into the sampling orifice of the atmospheric pressure interface of the time-of-flight mass spectrometer with the direct analysis in real time (DART) ion source operating in negative-ion mode. The mass spectra are dominated by peaks corresponding to [M + O₂]￣^?. No fragmentation is observed, making this a very soft ionization technique for samples that are otherwise difficult to analyze by DART. Detection limits for cholesterol were determined to be in the low nanogram range.

Fast and selective magnetic solid phase extraction of trace Cd, Mn and Pb in environmental and biological samples and their determination by ICP-MS

We have immobilized iminodiacetic acid on mesoporous Fe₃O₄@SiO₂ microspheres and used this material for efficient and cost effective method of magnetic solid phase extraction (SPE) of trace levels of Cd, Mn and Pb. The microspheres were characterized by infrared spectroscopy, scanning electron microscopy and transmission electron microscopy. The loaded microspheres can be easily separated from the aqueous sample solution by applying an external magnetic field. The effects of pH, sample volume, concentration and volume of eluent, and of interfering ions were investigated in detail. The method has detection limit of 0.16, 0.26 and 0.26?ng?L^?1 for the ions of Cd, Mn and Pb, respectively, and the relative standard deviations (RSDs, c?=?1???g?L^?1, n?=?7) are 4.8%, 4.6% and 7.4%. The method was successfully applied to the determination of these metals in biological and environmental samples using ICP-MS. Two certified reference materials were analyzed, and the results coincided well with the certified values.

Stereoselective (exo-specific) synthesis, dynamic 1H NMR and quantum chemical conformational and configurational analysis of norbornene-aziridine-E-imidoyl system

Stereoselective (exo-specific) synthesis, dynamic ¹H NMR and computational analysis of exo-N??-{3-azatricyclo[3.2.1.0.^2,4]oct-3-yl)mesithyloxy)methylene}-1-benzensulfunamide (3) were investigated. Aziridine nitrogen inversion gives rise to two sets of configurations where the N-substituent is Syn (S) or Anti (A) to C7 of the norbornyl ring. At lower temperature, the proton signals of aziridine exo-E-3 decoalesces to show two syn conformers and one anti conformer (exo-E-3 ^{1 S} ? $ \leftrightharpoons $ ?exo-E-3 ^{2 S} ? $ \leftrightharpoons $ ?exo-E-3 ^{3 A} ) with ratio of 60:20:20, respectively. Experimentally, the Gibbs free energy of activations [??G ^? (kcal/mol) ?±?0.08] were calculated 11.96, 12.45 for 3 isomerizations. The standard Gibbs free energy (??G ^o kcal/mol) 0.174, 0, 0.174, and 0.298 at 213?K and energy minimum 6.64, 4.77 and 1.78 were calculated for 3 ^1S? $ \leftrightharpoons $ ?3 ^2S, 3 ^2S? $ \leftrightharpoons $ ?3 ^{3 A} , 3 ¹ S? $ \leftrightharpoons $ ?3 ^{3 A} isomerizations, respectively. The enthalpy (??H ^?, kcal/mol) and entropy (??S ^?, cal?mol^?1?K^?1) of activation for the nitrogen inversion of aziridine of 3 were calculated 11.2 and ?0.80, respectively.     

Gas-phase chemiluminescent determination of inorganic selenium in water samples following flow injection hydride generation and cryotrapping

We describe a method for the determination of inorganic selenium in water samples via gas-phase chemiluminescence (GPCL). Se(IV) was first derivatized with 4-nitro-o-phenylenediamine to form 5-nitropiazselenol. The latter was decomposed by persulfate through photocatalytic oxidation to give Se(VI), which was reduced to Se(IV). Selenium hydride was generated from Se(IV) through reduction with sodium borohydride and then preconcentrated using cryotrapping. The cryotrapped hydride was evaporated and carried to a reaction chamber by a stream of helium, where it produced GPCL as a result of ozonation. The method exhibits a wide linear calibration range (from 0.5?μg?L^?1 to 1.0?mg?L^?1) with a detection limit of 0.12?μg?L^?1 (for n?=?11), and a relative standard deviation of 3.90?% (at n?=?11) at 5.0?μg?L^?1 level of selenium. The method was applied to the determination of inorganic selenium in water samples and gave satisfactory results.

Synthesis, crystal structures, and luminescence spectra of the coordination compounds of cadmium(II) iodide with hexamethylenetetramine

Coordination compounds [Cd_1.5I₃(HMTA) · H₂O] (I) and [CdI₂(HMTA) · H₂O] (II) are synthesized by the reaction of CdI₂ with hexamethylenetetramine (HMTA, C₆H₁₂N₄) with the 1: 1 ratio in ethanol, and their structures are determined. The crystals of compound I are triclinic, space group P $ \bar 1 $ , a = 8.027(1), b = 9.391(1), c = 10.382(1)?, ?? = 66.64(1)°, ?? = 86.18(1)°, ?? = 73.63(1)°, V = 749.2(1) ?³, ??_calcd = 3.136 g/cm³, Z = 2. The crystals of compound II are triclinic, space group P $ \bar 1 $ , a =7.713(1), b = 8.192(1), c = 12.101(1)?, ?? = 80.32(1)°, ?? = 89.57(1)°, ?? = 7.30(1)°, V = 725.0(1) ?³, ??_calcd = 2.402 g/cm³, Z = 2. Structure I includes two types of cadmium complexes. The Cd(1) atom is coordinated through the octahedral mode by three pairs of the I, N(HMTA), and O(H₂O) atoms. The coordination polyhedron of the Cd(2) atom is a distorted tetrahedron (three I atoms and one N atom). The structure contains infinite strips consisting of tetranuclear cyclic fragments joined by the Cd(1) atoms due to the bridging iodine and nitrogen atoms. In structure II, the Cd atom is coordinated through the tetrahedral mode by two iodide ions and the N(HMTA) and O(H₂O) atoms. The interaction between the complexes occurs due to hydrogen bonds O-H??N to form supramolecular chains along the direction [010]. In each HMTA molecule, one of four nitrogen atoms is a proton acceptor in the hydrogen bonds, one nitrogen atom is coordinated, and two N atoms are terminal. Compound II in the solid state has photoluminescence with maxima at 443, 470, and 518 nm.     

Direct electrochemistry of myoglobin in a layer-by-layer film on an ionic liquid modified electrode containing CeO2 nanoparticles and hyaluronic acid

We describe an ionic liquid modified electrode (CPE-IL) for sensing hydrogen peroxide (HP) that was modified by the layer-by-layer technique with myoglobin (Mb). In addition, the surface of the electrode was modified with CeO₂ nanoparticles (nano-CeO₂) and hyaluronic acid. UV-vis and FTIR spectroscopy confirmed that Mb retains its native structure in the composite film. Scanning electron microscopy showed that the nano-CeO₂ closely interact with Mb to form an inhomogeneously distributed film. Cyclic voltammetry reveals a pair of quasi-reversible redox peaks of Mb, with the cathodic peak at ?0.357?V and the anodic peak at ?0.269?V. The peak separation (??E _p) and the formal potential (E ^0??) are 88?mV and ?0.313?V (vs. Ag/AgCl), respectively. The Mb immobilized in the modified electrode displays an excellent electrocatalytic activity towards HP in the 0.6 to 78.0???M concentration range. The limit of detection is 50?nM (S/N?=?3), and then the Michaelis-Menten constant is 71.8???M. We believe that such a composite film has potential to further investigate other redox proteins and in the fabrication of third-generation biosensors.

Polyampholyte-tuned lyotrop lamellar liquid crystalline systems

The influence of a polyampholyte, i.e., poly(N,N′-diallyl-N,N′-dimethyl-altmaleamic carboxylate) (PalH), on the lamellar liquid crystalline (LC) system sodium dodecyl sulfate (SDS)/decanol/water was investigated by means of microdifferential scanning calorimetry, small-angle X-ray diffraction (SAXS), and cryo-scanning electron microscopy. After incorporating PalH into the lamellar liquid crystalline system, SAXS measurements show that three different LC phases exist: i.e., a swelling, slightly swelling, and non-swelling one. At pH 4, the positively charged polymer with an extended conformation can directly adsorb at the anionic head groups of the surfactant and more compact vesicles are formed at room temperature. At pH 9, the electrostatic interactions between the polyampholyte (in a more coiled conformation) and the sulfate head groups of the SDS are leveled off and incompact vesicles are formed at room temperature. That means in presence of the polyampholyte the morphology of the LC phase, i.e., the supramolecular vesicle structure, can be tuned by varying the pH and/or the temperature.

Structures and bonding situation of Pb2X2 (X?=?H, F, Cl, Br and I)

Quantum chemical calculations using DFT (BP86) and ab initio methods (MP2, MP4 and CCSD(T)) have been carried out for the title compounds. The nature of the Pb?CPb interactions has been investigated with an energy decomposition analysis. The energy minimum structures of the halogen substituted Pb₂X₂ molecules possess a doubly bridged butterfly geometry A like the parent system Pb₂H₂. The unusual geometry can be explained with the interactions between PbX fragments in the X ²?? ground state which leads to one Pb?CPb electron-sharing ?? bond and two donor?Cacceptor bonds between the Pb?CX bonds as donor and vacant p(??) AOs of Pb. The energy difference between the equilibrium form A and the linear structure XPb??PbX (E) which is a second-order saddle point is much higher when X is a halogen atom than for X?=?H. This is because the a ⁴??^?????X ²?? excitation energies of PbX (X?=?F?CI) are higher than for PbH. The structural isomers B, D1, D2, E, F1, F2 and G of Pb₂X₂ are no minima on the potential energy surface.     

Development of monolith-based stir bar sorptive extraction and liquid chromatography tandem mass spectrometry method for sensitive determination of ten sulfonamides in pork and chicken samples

A highly sensitive method was developed for the simultaneous determination of ten sulfonamides in pork and chicken samples by monolith-based stir bar sorptive extraction (SBSE) coupled to high-performance liquid chromatography tandem mass spectrometry. The samples were freeze-dried and extracted by acetonitrile, then enriched and further extracted by SBSE which was based on poly(vinylphthalimide-co-N,N-methylenebisacrylamide) monolith (SBSE-VPMB) as coating. To achieve optimum extraction performance of SBSE for sulfonamides, several parameters, including pH value and ionic strength in the sample matrix and extraction and desorption time, were investigated in detail. Under the optimal conditions, the limits of detection (S/N?=?3) for target sulfonamides were 1.2–6.1 ng/kg in pork and 2.0–14.6 ng/kg in chicken, respectively. Real samples spiked at the concentration of 0.5 and 5.0 μg/kg showed recoveries above 55 % and relative standard deviations below 12 %. At the same time, the extraction performances of target sulfonamides on SBSE-VPMB were compared with other SBSE based on porous monolith and commercial SBSE.

Metabolomic profiling of mice urine and serum associated with trans-trans 2, 4-decadienal induced lung lesions by liquid chromatography-mass spectrometry

Metabolomics has become an important tool in clinical research and the diagnosis of human disease. Intratracheal instillation of trans-trans 2,4-decadienal (tt-DDE), a major component in cooking oil fumes, has been demonstrated to cause lung lesions in mice at 8 weeks after treatment. The objective of this study was to identify any changes in metabolite profiles associated with the development of tt-DDE-induced lung lesions. Using a metabolomics strategy involving a liquid chromatography–mass spectrometry-based approach in conjunction with principal component analysis and confirmation by liquid chromatography triple quadrupole tandem mass spectrometry, we have demonstrated that the amino acid profiles of the urine and serum of tt-DDE-treated mice are changed. Ten amino acids were significantly reduced in serum of tt-DDE-treated mice at 8 weeks after treatment. Our results suggest that amino acid profiles may be useful as an early indicator of the presence of tt-DDE-induced lung lesions.

Synthesis of multi-branched gold nanoparticles by reduction of tetrachloroauric acid with Tris base, and their application to SERS and cellular imaging

A biosensor for hydrogen peroxide was constructed by immobilizing horseradish peroxidase on chitosan-wrapped NiFe₂O₄ nanoparticles on a glassy carbon electrode (GCE). The electron mediator carboxyferrocene was also immobilized on the surface of the GCE. UV?Cvis spectra, Fourier transform IR spectra, scanning electron microscopy, and electrochemical impedance spectra were acquired to characterize the biosensor. The experimental conditions were studied and optimized. The biosensor responds linearly to H₂O₂ in the range from 1.0?×?10^?5 to 2.0?×?10^?3?M and with a detection limit of 2.0?×?10^?6?M (at S/N?=?3).

ESI Mass Spectrometric Exploration of Selective Recognition of G-Quadruplex in c-myb Oncogene Promoter Using a Novel Flexible Cyclic Polyamide

In this research, electrospray ionization mass spectrometry (ESI-MS) was used to probe the binding selectivity of a flexible cyclic polyamide (cβ) to G-quadruplexes from the long G-rich sequences in the c-myb oncogene promoter. The results show that three G-rich sequences, including d[(GGA)₃GGTCAC(GGA)₄], d[(GGA)₄GAA(GGA)₄], and d[(GGA)₃GGTCAC(GGA)₄GAA(GGA)₄] species in the c-myb promoter can form parallel G-quadruplexes, and cβ selectively binds towards these G-quadruplexes over both several other G-quadruplexes and the duplex DNA. These properties of cβ have profound implications on future studies of the regulation of c-myb oncogene expression.

The reaction of ammonium tetra(isothiocyanato)diamminechromate(III) with ?-caprolactam in aqueous solution. Revised refinement of the structure of (HCpl2)3[Cr(NCS)6]

A reaction of ammonium tetra(isothiocyanato)diamminechromate(III) (ammonium reineckate) with ?-caprolactam in aqueous solution at different pH values gave the novel complexes (NH₄)[Cr(NH₃)₂(NCS)₄] · 7Cpl (I), (NH₄)[Cr(NH₃)₂(NCS)₄] · 2.5Cpl · 0.5(H₂O) (II), and (HCpl₂)[Cr(NH₃)₂(NCS)₄] (III), where Cpl is ?-caprolactam (?-C₆H₁₁NO). The crystals of complexes I?CIII are triclinic, space group $P\bar 1$ ; I: a = 12.7058(4) ?, b = 13.2544(4) ?, c = 19.4487(7) ?, ?? = 105.2360(10)°, ?? = 106.6410(10)°, ?? = 91.5290(10)°, V = 3009.37(17) ?³, ??_calc = 1.245 g/cm³, Z = 2; II: a = 12.3144(5) ?, b = 12.6518(5) ?, c = 23.3300(8) ?, ?? = 75.4580(10)°, ?? = 80.0760(10)°, ?? = 61.0830(10)°, V = 3074.1(2) ?³, ??_calc = 1.358 g/cm³, Z = 4; III: a = 6.4701(4) ?, b = 12.5973(9) ?, c = 16.5556(12) ?, ?? = 108.769(2)°, ?? = 98.543(2)°, ?? = 90.345(2)°, V = 1261.36(15) ?³, ??_calc = 1.437 g/cm³, Z = 2. The structure refinement for (HCpl₂)₃[Cr(NCS)₆] (IV) was revised. Like complex III, complex IV contains the cation (HCpl₂)⁺ stabilized by a strong hydrogen bond between the O atoms of the ?-caprolactam molecules; the cation was structurally characterized for the first time.