IR, Raman and SERS studies of methyl salicylate

The IR and Raman spectra of methyl salicylate (MS) were recorded and analysed. Surface enhanced Raman scattering (SERS) spectrum was recorded in silver colloid. The vibrational wave numbers of the compound have been computed using the Hartree-Fock/6-31G* basis and compared with the experimental values. SERS studies suggest a flat orientation of the molecule at the metal surface.     

Thermochemical and kinetic studies on the effects of cobalt salicylate on the oxidative degradation of polystyrene

The effect of cobalt salicylate on the oxidative degradation and ignition of polystyrene has been studied. It was found that cobalt salicylate sensitizes both the degradation and ignition of polystyrene by facilitating electron-transfer processes in the propagation step. From thermochemical and kinetic studies it was found that the cobalt ion, owing to its ability to exist in variable valence states, promotes electron transfer in the propagation step of polymer degradation, increasing the rate of propagation and consequently the overall rate. Using solid-phase thermal ignition theory, an attempt has been made to explain the sensitization of ignition by the cobalt ion.

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Zusammenfassung Die Wirkung von Kobaltsalicylat auf den oxydativen Abbau und die Entzündung von Polystyrol wurde untersucht. Es wurde festgestellt, daß Kobaltsalicylat sowohl den Abbau als auch die Entzündung des Polystyrols durch Erleichterung von Elektrontransferprozessen im Kettenfortpflanzungsschritt begünstigt. Thermochemische und kinetische Untersuchungen ergeben, daß das Kobaltion infolge seiner Fähigkeit, in mehreren Valenzstufen aufzutreten, den Elektronentransfer im Kettenfortpflanzungsschritt erleichtert wodurch die Geschwindigkeit der Kettenfortpflanzung und damit die Geschwindigkeit des Gesamtprozesses erhöht wird. Basierend auf der Theorie der thermischen Festphasenentzündung wird ein Versuch unternommen, Erleichterung der Entzündung durch Kobaltionen zu erklären.

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Interaction of manganese(II) with methyl salicylate ethyl salicylate and phenyl salicylate

The proton ligand stability constants of methyl salicylate, ethyl salicylate and phenyl salicylate and the stepwise stability constants of manganese(II) complexes with these have been determined potentiometrically in aqueous ethanol system 50/50 (v/v) at 25°C at different ionic strengths, viz. 0.050 M, 0.075 M, 0.100 M and at 35 and 45°C at an ionic strength of 0.05 M. The thermodynamic stability constants of the complexes have been evaluated from the various values by extrapolating to zero ionic strength at 25°C. The thermodynamic parameters such as free energy changes (ΔG), enthalpy changes (ΔH) and entropy changes (ΔS) involved have been calculated.     

Liquid-liquid distribution studies of thorium salicylate with tris-(2-ethylhexyl)phosphate

A method is proposed for the extraction of thorium(IV) from salicylate media using tris-(2-ethylhexyl)phosphate dissolved in toluene as an extractant. The optimum conditions were evaluated from a critical study of pH, salicylate concentration, extractant concentration, period of equilibration and diluent. The method permits the separation of thorium from the associated elements and is applicable to the analysis of monazite sand. The method is precise, accurate, fast and selective.     

Inhibition of Escherichia coli porphobilinogen synthase using analogs of postulated intermediates

BACKGROUND: Porphobilinogen synthase is the second enzyme involved in the biosynthesis of natural tetrapyrrolic compounds, and condenses two molecules of 5-aminolevulinic acid (ALA) through a nonsymmetrical pathway to form porphobilinogen. Each substrate is recognized individually at two different active site positions to be regioselectively introduced into the product. According to pulse-labeling experiments, the substrate forming the propionic acid sidechain of porphobilinogen is recognized first. Two different mechanisms for the first bond-forming step between the two substrates have been proposed. The first involves carbon-carbon bond formation (an aldol-type reaction) and the second carbon-nitrogen bond formation, leading to an iminium ion. RESULTS: With the help of kinetic studies, we determined the Michaelis constants for each substrate recognition site. These results explain the Michaelis-Menten behavior of substrate analog inhibitors - they act as competitive inhibitors. Under standard conditions, however, another set of inhibitors demonstrates uncompetitive, mixed, pure irreversible, slow-binding or even quasi-irreversible inhibition behavior. CONCLUSIONS: Analysis of the different classes of inhibition behavior allowed us to make a correlation between the type of inhibition and a specific site of interaction. Analyzing the inhibition behavior of analogs of postulated intermediates strongly suggests that carbon-nitrogen bond formation occurs first.     

Inhibition of (+)-aristolochene synthase with iminium salts resembling eudesmane cation

Trigonal iminium halides of (4aS,7S)-1,4a-dimethyl- and (4aS,7S)-4a-methyl-7-(prop-1-en-2-yl)-2,3,4,4a,5,6,7,8-octahydroquinolinium ions, aimed to mimic transition states associated with the aristolochene synthase-catalyzed cyclization of (-)-germacrene A to eudesmane cation, were evaluated under standard kinetic steady-state conditions. In the presence of inorganic diphosphate, these analogues were shown to competitively inhibit the enzyme, suggesting a stabilizing role for the diphosphate leaving group in this apparently endothermic transformation.     

Immunochemical studies of the cellulose synthase complex inAcetobacter xylinum

An immunochemical method was used to analyse the 83 and 93 Kd polypeptides of cellulose synthase from Acetobacter xylinum.Polyclonal antibodies were raised against the LDS-PAGE-fractionated 83 and 93 Kd polypeptides isolated from A. xylinum.Using these antibodies, the 83 and 93 Kd polypeptides were localized in the different fractions during purification of cellulose synthase, and the ratio of these two polypeptides was determined to be 11. A differential solubilization of the 83 and 93 Kd polypeptides from the cell strongly suggested that the mechanism by which these two polypeptides originate from a single acsAB gene product (Saxena et al.,1994) must be via a post-translational cleavage. The results of trypsin treatment of the membrane fraction used in the purification of cellulose synthase were analysed to determine the fate of these two polypeptides and their relationship to the enzyme activity.     

Small-angle X-ray scattering studies on the X-ray induced aggregation of malate synthase I. Structural and kinetic studies

Small-angle X-ray scattering measurements on malate synthase in aqueous solution revealed a continuous increase of the intensity in the innermost portion of the scattering curve with increasing measuring time. We have definite evidence that this increase reflects an X-ray induced aggregation of the enzyme particles in the course of the small-angle X-ray scattering experiment. Obviously this aggregation is a consequence of a radiation damage of the particles by the primary beam used in the scattering experiment.The aggregation process of malate synthase was monitoredin situ by smallangle X-ray scattering. For this purpose scattering curves were taken at various stages of aggregation. The analysis of these curves established the increase of the particle dimensions, the retention of the pseudo thickness factor of the native enzyme and the occurrence of one and later on of two pseudo cross-section factors. These results suggest the way how the aggregation might proceed. The results led to a tentative model of the aggregation process in which a one-dimensional side-by-side association of the oblate enzyme particles is followed by a two-dimensional aggregation. An aggregation in the third dimension was not observed during the time covered by our experiment.The time dependence of molecular parameters, for instance of the apparent mean radius of gyration, was used to compare the aggregation of enzyme samples that were irradiated under different experimental conditions. The addition of dithiothreitol to the enzyme solutions as well as the presence of the substrates or of a substrate analogue or of ethanol were found to reduce the rate of aggregation.

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Röntgenkleinwinkeluntersuchungen der durch Röntgenstrahlen induzierten Aggregation der Malatsynthase. I. Strukturuntersuchungen und kinetische Messungen

Zusammenfassung Röntgenkleinwinkeluntersuchungen an wäßrigen Lösungen von Malatsynthase zeigten eine mit der Meßdauer ansteigende Zunahme der Streuintensität im Innenteil der Streukurve. Dieser Intensitätsanstieg spiegelt zweifelsohne eine durch die Röntgenbestrahlung induzierte Aggregation der Enzymteilchen während der Röntgenkleinwinkelmessung wider. Diese Aggregation ist offensichtlich auf einen durch die Primärstrahlung verursachten Strahlenschaden zurückzuführen.Das Fortschreiten der Aggregation der Malatsynthase wurde mit Hilfe der Röntgenkleinwinkelstreuungin situ verfolgt. Zu diesem Zweck wurden Streukurven bei verschiedenen Aggregationsstadien aufgenommen. Die Analyse dieser Kurven zeigte die Zunahme der Teilchendimensionen, das Beibehalten des Pseudodickenfaktors des nativen Enzyms und das Auftreten eines und später zweier Pseudoquerschnittsfaktoren an. Diese Ergebnisse lieferten Hinweise, wie die Aggregation ablaufen könnte, und führten zu einem möglichen Modell für den Aggregationsvorgang. Demnach sollte auf eine eindimensionale, laterale Aggregation der oblaten Enzymteilchen eine zweidimensionale Aggregation folgen. Ein Fortschreiten der Aggregation in der dritten Dimension konnte während der Dauer des Experimentes nicht beobachtet werden.Die zeitliche Abhängigkeit molekularer Parameter, z. B. des apparenten mittleren Streumassenradius, wurde für den Vergleich der Aggregation von Enzymproben, die unter verschiedenen experimentellen Bedingungen bestrahlt wurden, herangezogen. Durch Zugabe von Dithiothreitol oder Ethanol zu den Enzymlösungen oder durch die Anwesenheit der Substrate oder eines Substratanalogen konnte die Aggregationsgeschwindigkeit herabgesetzt werden.

     

Kinetic and theoretical studies on alkaline ethanolysis of 4-nitrophenyl salicylate: effect of alkali metal ions on reactivity and mechanism

Pseudo-first-order rate constants (k(obsd)) for reactions of 4-nitrophenyl salicylate (7) with alkali metal ethoxides (EtOM, M = K, Na, and Li) in anhydrous ethanol have been measured spectrophotometrically. Interestingly, the k(obsd) value decreases significantly as the concentration of EtOM increases. Because the phenolic moiety of substrate 7 would be deprotonated and exist as an anionic form (i.e., 7(-)) under kinetic conditions, the ground-state stabilization of 7(-) through formation of a six-membered cyclic complex with M(+) (i.e., 8) is proposed to be responsible for the decreasing k(obsd) trend. The k(obsd) value at a given concentration of EtOK increases steeply upon addition of [18]crown-6 ether (18C6) up to [18C6]/[EtOK] = 1 in the reaction mixture and then remains relatively constant thereafter. In contrast, k(obsd) decreases upon addition of salts (e.g., LiClO(4) or KSCN) to the reaction mixture, which indicates that M(+) ions inhibit the reaction. However, in the presence of 18C6, the k(obsd) value is independent of the concentration of EtOK but remains constant, which indicates that the reaction proceeds through a unimolecular mechanism in the presence of the complexing agent. Although two conceivable unimolecular pathways (formation of ketene 9 and lactone 10) can account for the kinetic results, the reaction has been concluded to proceed via formation of ketene 9 as the reactive intermediate on the basis of theoretical calculations.     

Thermal analysis,synthesis and structural studies of heterometallic {Fe2MO} salicylate complexes

Journal of Thermal Analysis and Calorimetry - Four new trinuclear heterometallic molecular complexes with the {Fe2IIIMII μ3-O} core, where M?=?Mn(II), Ni(II), Cu(II) and Zn(II),...     

Determination of salicylate in blood serum by flow injection with immobilized salicylate hydroxylase

A flow injection (FI) enzymatic system, based on the use of immobilized salicylate hydroxylase in glass beads, was developed for the determination of salicylate. Salicylate hydroxylase and nicotinamide adenine dinucleotide (NADH) are used to convert salicylate to catechol. The reaction of catechol with 4-aminophenol at high pH yields a colored product which is detected spectrophotometrically at 565 nm. Ten samples of human serum containing from 5.0 x 10(-4) to 5.0 x 10(-3) mol/L added salicylate were analyzed and the recovery was determined. Eight additional serum samples containing salicylate were analyzed by the Trinder test and the proposed method. The results obtained with the 2 methods showed good agreement by the statistical Student's t-test. The relative precision of the method is about 3.4% (RSD of the mean recovery). Considering the lowest concentration analyzed, the quantitative limit of detection is about 0.2 x 10(-5) mol/L (3 x SD). The volume of the sample used was 150 microL. The proposed method was also used to analyze medicines containing acetylsalicylic acid. The results were statistically compared with those obtained through the U.S. Pharmacopoeia procedure and showed excellent agreement.     

Catecholate/salicylate heteropodands: demonstration of a catecholate to salicylate coordination change

While iron release from enterobactin-mediated iron transport occurs primarily via an esterase that destroys the siderophore, other catechol siderophores that are not susceptible to hydrolysis act as bacterial growth factors. Elucidating the structures of protonated ferric enterobactin may reveal the pathway by which synthetic analogues fulfill bacterial iron requirements. In order to more completely model this potential delivery pathway for ferric iron, as well as to understand the pH dependent structural dynamics of ferric enterobactin, two ligands, (2-hydroxybenzoyl-2-aminoethyl)-bis(2,3-dihydroxybenzoyl-2-aminoethyl)amine (TRENCAMSAM) and (2-hydroxy-3-methoxybenzoyl-2-aminoethyl)-bis(2,3-dihydroxybenzoyl-2- aminoethyl)amine (TRENCAM(3M)SAM), have been synthesized as models for monoprotonated enterobactin. The coordination chemistry of these ligands with Fe3+ and Al3+ has been investigated. Fe[TRENCAMSAM]2- crystallizes in the triclinic space group P1: Z = 1, a = 11.3307(6) A, b = 12.5479(7) A, c = 15.5153(8) A, alpha = 94.513(1) degree, beta = 105.867(1) degree, gamma = 94.332(1) degree. The structure is a two-metal two-ligand dimer supported by mu-oxo bridges from two catecholate moieties. Al[TRENCAMSAM]2- crystallizes in the triclinic space group P1: Z = 2, a = 9.1404(2) A, b = 13.3570(1) A, c = 15.5950(1) A, alpha = 95.711(1) degree, beta = 104.760(1) degree, gamma = 92.603(1) degree. The complex is a monomer with a five-coordinate, square-pyramidal aluminum cation. Al[TRENCAM(3M)SAM]2- crystallizes in the monoclinic space group C2/m: Z = 8, a = 34.244(2) A, b = 11.6206(6) A, c = 21.9890(12) A, beta = 101.478(1) degree. The complex is also a monomer, but with a highly distorted five-coordinate, square-pyramidal aluminum cation coordination sphere. At high pH these complexes do not display a salicylate mode of binding; however, at low pH Al[TRENCAMSAM]2- converts to protonated Al[H3TRENCAMSAM]+, which is a six-coordinate, tris-salicylate complex. Al[H3TRENCAMSAM]+ crystallizes in the triclinic space group P1: Z = 2, a = 11.5475(4) A, b = 12.1681(4) A, c = 12.5094(4) A, alpha = 109.142(1) degree, beta = 104.327(1) degree, gamma = 103.636(1) degree. This is the first catecholamide enterobactin analogue that has been structurally characterized in both a catecholate and salicylate mode of coordination.     

中性载体水杨酸根离子电极的研究

近年来,反Hofmeister行为的阴离子选择性电极的研究是离子电极研究领域中重要的研究方向之一[1],其中许多平面结构的Schiff碱金属配合物对特种阴离子表现较高选择性,以此研制了许多高选择性I-电极[2,3]、S al-电极[4-6]、SCN-电极[7,8].     

Crystallographic studies on the reaction of isopenicillin N synthase with an unsaturated substrate analogue

Isopenicillin N synthase (IPNS) catalyses conversion of the linear tripeptide delta-(L-alpha-aminoadipoyl)-L-cysteinyl-D-valine (ACV) to isopenicillin N (IPN), the central step in biosynthesis of the beta-lactam antibiotics. The unsaturated substrate analogue delta-(L-alpha-aminoadipoyl)-L-cysteinyl-D-vinylglycine (ACvG) has previously been incubated with IPNS and single product was isolated, a 2-alpha-hydroxymethyl isopenicillin N (HMPen), formed via a monooxygenase mode of reactivity. ACvG has now been crystallised with IPNS and the structure of the anaerobic IPNS:Fe(II):ACvG complex determined to 1.15 A resolution. Furthermore, by exposing the anaerobically grown crystals to high-pressure oxygen gas, a structure corresponding to the bicyclic product HMPen has been obtained at 1.60 A resolution. In light of these and other IPNS structures, and recent developments with related dioxygenases, the [2 + 2] cycloaddition mechanism for HMPen formation from ACvG has been revised, and a stepwise radical mechanism is proposed. This revised mechanism remains consistent with the observed stereospecificity of the transformation, but fits better with apparent constraints on the coordination geometry around the active site iron atom.     

Determination of salicylate in blood serum using an amperometric biosensor based on salicylate hydroxylase immobilized in a polypyrrole-glutaraldehyde matrix

The use of an amperometric biosensor for the salicylate determination in blood serum is described. The biosensor is based on salicylate hydroxylase (EC 1.14.13.1) electropolymerized onto a glassy carbon-working electrode with polypyrrole and glutaraldehyde, to improve the biosensor lifetime. The hexacyanoferrate (II) was also incorporated to work as a redox mediator to minimize possible interferences. The salicylate is enzymatically converted to catechol, which is monitored amperometrically by its electrooxidation at+0.170 V versus SCE (saturated calomel electrode). Salicylate determination was carried out maintaining the ratio between beta-NADH and salicylate at 4:1 (30 degrees C). The amperometric response of the biosensor was linearly proportional to the salicylate concentration between 2.3x10(-6) and 1.4x10(-5) mol l(-1), in 0.1 mol l(-1) phosphate buffer (pH 7.8), containing 0.1 mol l(-1) KCl and 5.0x10(-4) mol l(-1) Na(2)H(2)EDTA, as supporting electrolyte. The recovery studies, in the presence of several interfering compounds, showed recoveries between 96.4 and 104.8%. The useful lifetime of the biosensor in the concentration range evaluated was at least 40 days, in continuous use. Blood serum samples analyzed by this biosensor showed a good correlation compared to the spectrophotometric method (Trinder) used as reference, presenting relative deviations lower than 7.0%.     

Transesterification kinetics of phenyl salicylate

The degradation of phenyl salicylate in alkaline aqueous ethanol is shown to proceed via competing transesterification and hydrolysis processes. The transesterified product, ethyl salicylate, also undergoes hydrolysis, but at a slower rate and a kinetic model is presented which allows the simultaneous determination of all three rate constants. These results are contrasted with those of an earlier literature study and show the necessity for specific assay systems in kinetic analysis.     

Evaluation of potential inhibitors of squalene synthase based on virtual screening and in vitro studies

Squalene synthase (SQS) is a potential target for hyperlipidemia treatment. To identify novel chemical scaffolds of SQS inhibitors, we generated 3D-QSAR pharmacophore models using HypoGen. The best quantitative pharmacophore model, Hypo 1, was selected for virtual screening using two chemical databases, Specs and Traditional Chinese Medicine database (TCM). The best-mapped hit compounds were then subjected to filtering by Lipinski^’s rule of five and docking studies to refine the hits. Finally, five compounds were selected from the top-ranked hit compounds for SQS inhibitory assay in vitro. Three of these compounds could inhibit SQS in vitro, and should be further evaluated pre-clinically as a treatment for hyperlipidemia.