We have evaluated the abilities of ferulic acid, (±) catechin, (+) catechin and (-) epicatechin to scavenge the reactive oxygen species hydroxyl radical (OH±), hypochlorous acid (HOCl) and peroxyl radicals (RO2).Ferulic acid tested at concentrations up to 5 mM inhibited the peroxidation of phospholipid liposomes. Both (±) and (+) catechin and (-) epicatechin were much more effective. All the compounds tested reacted with trichloromethyl peroxyl radical (CCl3O2) with rate constants > 1 × 106M?1s?1.A mixture of FeCl3-EDTA, hydrogen peroxide (H2O2) and ascorbic acid at pH 7.4, has often been used to generate hydroxyl radicals (OH.) which are detected by their ability to cause damage to the sugar deoxyribose. Ferulic acid, (+) and (±) catechin and (-) epicatechin inhibited deoxyribose damage by reacting with OH. with rate constants of 4.5 × 109M?1s?1, 3.65 × 109M?1s?1, 2.36 × 109M?1s?1 and 2.84 × 109M?1s?1 respectively. (-) Epicatechin, ferulic acid and the (+) and (±) catechins exerted pro-oxidant action, accelerating damage to DNA in the presence of a bleomycin-iron complex. On a molar basis, ferulic acid was less effective in causing damage to DNA compared with the catechins.A mixture of hypoxanthine and xanthine oxidase generates O2 which reduces cytochrome c to ferrocytochrome c. (+) Catechin and (-) epicatechin inhibited the reduction of cytochrome c in a concentration dependent manner. Ferulic acid and (±) catechin had only weak effects.All the compounds tested were able to scavenge hypochlorous acid at a rate sufficient to protect alpha-1-antiproteinase against inactivation. Our results show that catechins and ferulic acid possess antioxidant properties. This may become important given the current search for “natural” replacements for synthetic antioxidant food additives. 相似文献
The preparation of the planar yellow [Ni([8]aneN2)2](ClO4)2 is described. The complex dissociates in basic solution, with rate = kOH[NiL][OH?] (L = 1,5-diazacyclo-octane). At 25 °C, kOH = 4.5 x 10?2 M?1 s?1 and the corresponding activation parameters are ΔH≠ = 69.2 kJ mol?1 and ΔS298≠ = ?38.6 J K?1 mol?1. Acid catalysed dissociation in quite slow even in strongly acidic solutions. The kinetic data in this case can be fitted to the expression Kobs = ko + KH[H+], where ko relates to a solvolytic pathway and kH to the acid catalysed pathway. At 60 °C, Ko = 2 x 10?5 s?1 and kH is 2 x 10?5 M?1 s?1. Possible mechanisms for these reactions are considered.The Ni(II)/Ni(III) redox couple for NiLn+ is irreversible on Pt using MeCN as solvent. 相似文献
Nongelling solutions of structurally regular chain segments of agarose sulphate show disorder–order and order–disorder transitions (as monitored by the temperature dependence of optical rotation) that are closely similar to the conformational changes that accompany the sol–gel and gel–sol transitions of the unsegmented polymer. The transition midpoint temperature (Tm) for formation of the ordered structure on cooling is ~25 K lower than Tm for melting. Salt-induced conformational ordering, monitored by polarimetric stopped-flow, occurs on a millisecond time scale, and follows the dynamics expected for the process 2 coil ? helix. The equilibrium constant for helix growth (s) was calculated as a function of temperature from the calorimetric enthalpy change for helix formation (ΔHcal = ?3.0 ± 0.3 kJ per mole of disaccharide pairs in the ordered state), measured by differential scanning calorimetry. The temperature dependence of the nucleation rate constant (knuc), calculated from the observed second-order rate constant (kobs) by the relationship kobs = knuc(1 ? 1/s) gave the following activation parameters for nucleation of the ordered structure of agarose sulphate (1 mg mL?1; 0.5M Me4NCl or KCl): ΔH* = 112 ± 5 kJ mol?1; ΔS* = 262 ± 20 J mol?1 K?1; ΔG*298 = 34 ± 6 kJ mol?1; (knuc)298 = (7.5 ± 0.5) × 106 dm3 mol?1 s?1. The endpoint of the fast relaxation process corresponds to the metastable optical rotation values observed on cooling from the fully disordered form. Subsequent slow relaxation to the true equilibrium values (i.e., coincident with those observed on heating from the fully ordered state) was monitored by conventional optical rotation measurements over several weeks and follows second-order kinetics, with rate constants of (2.25 ± 0.07) × 10?4 and (3.10 ± 0.10) × 10?4 dm3 mol?1 s?1 at 293.7 and 296.2 K, respectively. This relaxation is attributed to the sequential aggregation processes helix + helix → dimer, helix + dimer → trimer, etc., with depletion of isolated helix driving the much faster coil–helix equilibrium to completion. Light-scattering measurements above and below the temperature range of the conformational transitions indicate an average aggregate size of 2–3 helices. 相似文献
Pentaammineruthenium(III) complexes of deoxyinosine (dIno) and xanthosine (Xao) ([RuIII(NH3)5(L)], L?is?dIno, Xao) in basic solution were studied by UV?Cvis spectroscopy, liquid chromatography/electrospray ionization mass spectrometry, and high-performance liquid chromatography. Both RuIII complexes disproportionate to RuII and RuIV. Disproportionation followed the rate law d[RuII]/dt?=?(ko?+?k1[OH?])[RuIII]. ko and k1 of disproportionation at 25?°C were 2.1 (±0.1)?×?10?3?s?1 and 21.4?±?3.2?M?1 s?1, respectively, for [RuIII(NH3)5(dIno)], and 3.5 (±0.7)?×?10?4?s?1 and 59.7?±?3.6?M?1?s?1, respectively, for [RuIII(NH3)5(Xao)]. The [RuIII(NH3)5(Xao)] complex disproportionates at a faster rate than [RuIII(NH3)5(dIno)] owing to the stronger electron-withdrawing effect of exocyclic oxygen in Xao. The activation parameters ??H? and ??S? for k1 of [RuIII(NH3)5(dIno)] were 80.2?±?15.2?kJ?mol?1 and 47.6?±?9.8?J?K?1 mol?1, respectively, indicating that the disproportionation of RuIII to RuII and RuIV is favored owing to the positive entropy of activation. The final products of both complexes in basic solution under Ar were compared with those under O2. Under both conditions [Ru(NH3)5(8-oxo-L)] was produced, but via different mechanisms. In both aerobic and anaerobic conditions, the deprotonation of highly positively polarized C8-H of Ru-L by OH? initiates a two-electron redox reaction. For the next step, we propose a one-step two-electron redox reaction between L and RuIV under anaerobic conditions, which differentiates from Clarke??s mechanism of two consecutive one-electron redox reactions between L, RuIII, and O2. 相似文献
Pulse radiolysis-kinetic spectrometry has been used to investigate the reaction of hydrated electrons with ferricytochrome c in dilute aqueous solution at pH 6.5–7.0. Time resolutions from 2·10?7 to 1 s were employed. Transient spectra from 320 to 580 nm were characterized with a wavelength resolution of ±0.5 nm. 1 In neutral salt-free solution, k(ferricytochrome c+e?aq)=(6.0±0.9)·1010 M?1·s?1 and k(ferricytochrome c+H)=(1.2±0.2)·1010 M?1·s?1. The reaction of ferricytochrome c with hydrated electrons is sensitive to ionic strength; in 0.1 M NaClO4, k(ferricytochrome c+e?aq)=(2.4±0.4)·1010 M?1·s?1. In contrast, k(ferricytochrome c+H) is insensitive to ionic strength. Time resolution of three spectral stages has been accomplished. The primary spectrum is the first observable spectrum detectable after irradiation and is formed in a second-order process. Its rate of formation is indisting-uishable from the rate of disappearance of the electron spectrum. The secondary spectrum is generated in a true first order intramolecular process, k(p→s)=(1.2±0.1)·105 s?1. The tertiary spectrum is also generated in a true first-order process, k(s→t)=(1.3±0.2)·102 s?1. The specific rates of both transformations are independent of the wavelength of measurement. The tertiary spectrum, observable 50 ms after initial reaction and remaining unchanged thereafter for at least 1 s, shows that relaxed ferrocytochrome c is the only detectable product. This product is not autoxidizable, as expected for native reduced enzyme. It is more probable that the intramolecular changes responsible for the p→s and s→t spectral transformations involve the influence of conformational relaxation of ferrocytochrome c upon electronic energy states then that they are intramolecular transmission of reducing equivalents from primary sites of electron attachment. 相似文献
SummaryThe reaction between peroxynitrous acid (hydrogen oxoperoxonitrate) and L-tryptophan is 130 M?1s?1 at 25°C. The pH dependence of the second-order rate constant shows a maximum at pH 5.1. The enthalpy and entropy of activation at pH 7.1 are 10.6 ± 0.4 kcal.mol?1 and -16 ± 2 cal.mol?1K?1 respectively. High-performance liquid chromatography analysis revealed a number of reaction products, two of which were identified as 5- and 6- nitrotryptophan. Hydroxytryptophans were not observed, even at low peroxynitrite concentrations where most of the peroxynitrite decays to nitrate via a first-order process. These results support the hypothesis that isomerization of protonated peroxynitrite to nitrate does not involve formation of the hydroxyl radical. 相似文献
The rate constant for the reaction of NO with ·O2? was determined to be (6.7 ± 0.9) × 109 1 mol?1 s?1, considerably higher than previously reported. Rate measurements were made from pH 5.6 to 12.5 both by monitoring the loss of ·O2? and the formation of the product ?OONO. The decay rate of ?OONO, in the presence of 0.1 moll?1 formate, ranges from 1.2s?1 at pH 5 to about 0.2s?1 in strong base, the latter value probably reflecting catalysis by formate. 相似文献
Measurements of the equilibrium and temperature-jump u.v., visible, and induced c.d. spectra of Methyl Orange (MO) in the presence of cyclomalto-octaose (γ-cyclodextrin, γ-CD) have been carried out. Three mechanistic steps were detected through the temperature-jump data (25.0°): where K1, K2, and K3 are 45 (±7), 2.0 (±1.1) × 106, and 6.1 (±2.5) × 103 dm3.mol?1, respectively, k2 = 9.4 (±5.1) × 109 dm3.mol?1.s?1, and k?2 = 4.8 (±0.8) × 103 s?1. The equilibrium u.v./visible data are also consistent with this reaction scheme. The high stability of the dimer inclusion complex (MO)2 · γ-CD compared to that of the monomer inclusion complex MO · γ-CD appears to be related to the annular diameter of γ-CD and demonstrates a degree of selectivity in cyclodextrin inclusion complexes. The (MO)2 · (γ-CD)2 complex also contains a dimer, included by both γ-CD molecules. 相似文献
The interactions between cytochrome P450 2B4 (d-2B4), NADPH:cytochrome P450 reductase and cytochrome b5 have been investigated in the monomeric reconstituted P450 2B4-containing monooxygenase system in the presence of a substrate (7-pentoxyresorufin) and an electron donor, NADPH. Each partner was immobilized via its amino groups on the carboxymethyldextran biochip surface of the optical biosensor IAsys+. Such mode immobilization was not accompanied by any loss of activities of the immobilized proteins. The formation of binary d-Fp/d-2B4 complexes was registered. The association/dissociation rate constants (kon/koff) were (0.013 ± 0.005) × 106 M?1 s?1/0.05 ± 0.02 s?1, and dissociation constant (KD) was (0.26 ± 0.13) × 10?6 M. Comparison of kon, koff and KD values for d-Fp/d-2B4 complexes formed under hydroxylation (O-dealkylation) with corresponding constants obtained for the oxidized proteins of (0.10 ± 0.03) × 106 M?1 s?1/(0.14 ± 0.06) s?1, and (0.71 ± 0.37) × 10?6 M, respectively shows that the decrease in kon and an insignificant decrease in KD are associated with the increase of complex lifetime during transition from the oxidized to hydroxylation conditions. Complex formation between d-Fp and d-b5 was not registered in both hydroxylation conditions and in the case of oxidized forms of these proteins. In both cases formation of the ternary d-Fp/d-2B4/d-b5 complexes occurred. 相似文献
AbstractCordil-LND796 is a new cardiotonic glycoside under development. In rat brain microsomes where three isoforms of the Na, K-ATPase with differential affinities for cardiac glycosides have been identified, Cordil had higher affinity for the α3 (IC50 = 0.02 μM) than for the α2 (IC50 = 0.6 μM) and the α1 (IC50 = 30 μM) isozymes. Cordil is potentially a selective inhibitor for both α2 and α3 Na, K-ATPase isoforms. Using inside out vesicles we have shown that Cordil binds to and inhibits Na, K-ATPase at an extracellular site. The dissociation kinetic rates (k?1) from the ATPase and the phosphatase activity (K-dependent dephosphorylation) of the Na, K-ATPase were similar for Cordil. Despite these similarities to ouabain comparison of the kinetics of the Na, K-ATPase inhibition by ouabain and Cordil revealed marked differences in their association rates (k+1 = 0.7 1 mol1 min?1 and k+1 = 6 × 10?3 1 mol?1 min?1 respectively) and their dissociation rates (k?1 = 1.3 ± 0.2 × 10?4 S?1 and k?1 = 69 ± 7 × 10?4 s?1 respectively). Both binding association and dissociation rates were enhanced for Cordil. These data are compatible with a stabilizing effect of Cordil on the E2P conformational state of Na, K-ATPase. 相似文献
SummaryUsing the pulse radiolysis technique, absolute rate constants have been obtained for the reaction of captopril with several free radicals. The results demonstrate that although captopril reacts rapidly with a number of free radicals, such as the hydroxyl radical (k = 5.1 × 109 dm?3mol?1s?1) and the thiocyanate radical anion (k = 1.3 × 107 dm?3mol?1s?1), it is not exceptional in this ability. Similarly, the reactions with carbon centred radicals although rapid are an order of magnitude slower than those observed with glutathione. Additional lipid peroxidation studies further demonstrate that captopril is a much less effective antioxidant than glutathione. The data go some way to supporting the view that any attenuation of reperfusion injury by captopril is not through a direct free radical scavenging mechanism but may be afforded by other, non-radical-mediated mechanisms. 相似文献
AbstractObesity is prone to cause a variety of chronic metabolic diseases, and it has aroused people’s attention that the rapid increase in the global population of obese people in the past years. As a kind of weight-loss drug acting in the intestine, lipase inhibitor does not enter the bloodstream without producing central nervous side effects. Because they do not affect the metabolism system, lipase inhibitors and obesity have become one of the hot spots in recent years. Glycolic acid is a new substrate analog inhibitor with the value of the semi-inhibitory concentration of lipase is estimated to be 17.29?±?0.14?mM. Using the plots of Lineweaver-Burk, the inhibition mechanism of lipase by glycolic acid was reversible and the inhibition type belongs to competitive inhibition with a KI value of 19.61?±?0.26?mM. The inhibitory kinetics assay showed that the microscopic velocity constant k+0 of inhibition kinetics is 1.79?×?10?3?mM?1s?1, and k?0 is 0.73?×?10?3 s?1. The results of UV full-wavelength scanning on product cumulative, fluorescence quenching and molecular simulation also indicated that glycolic acid and substrate competitive with lipase by binding to Lys137. Thereby glycolic acid inhibiting the oxidation-catalyzed reaction and reducing the product of the enzyme and substrate. This adds a new direction for the search for lipase inhibitors and provides new ideas about the development of anti-obesity drugs.Communicated by Ramaswamy H. Sarma 相似文献
AbstractSaturation experiments were performed on intact human peripheral mononuclear leucocytes (MNL) and MNL membranes with (-)125Iodocyanopindolol (125ICYP) over a large concentration range (1.5-600pmol/l). The corresponding Scatchard plots were curvilinear suggesting two saturable classes of binding sites: A high affinity binding site (Bmax1=1000±400 sites/cell, Kd1= 2.1±0.9 pmol/l for intact MNL and Bmax1=550±190 sites/cell, Kd1=4.1±0.9 pmol/l for MNL membranes)and a low affinity binding site (Bmax2=9150±3590 binding sites/cell, Kd2=440±50 pmol/l for intact MNL and Bmax2=11560±4690 sites/cell, Kd2=410±70 pmol/l for MNL membranes). Dissociation of (-)125ICYP from MNL was biphasic consisting of a slow dissociating component (dissociation rate constant k-1=(0.5±0.2)x10?3 min?1 for intact MNL and k-1=(1.0±0.1)x10?3min?1 for MNL membranes) and a fast dissociating component (k-2=(80±20)x10?3min?1 for intact MNL and k-2=(60±10)x10?3min?1 for MNL membranes). In dissociation experiments started after equilibration with various (-)125ICYP concentrations k-1 and k-2 were independent of the equilibrium concentration, whereas the percentual occupancy of the slow and the fast dissociating component varied and was similar to the estimated fractional occupancy of either binding site at the same (-)125ICYP concentrations in saturation experiments. The association rate constant was in the same order of magnitude for both binding sites. These results suggest two independent classes of binding sites for (-)125ICYP on MNL. 相似文献
The thermal degradation kinetics of pectin methylesterase (PME) from carrot and lettuce were studied. Fresh extracts were exposed to temperatures from 55 to 70 °C until the enzyme was inactivated. A model based on the presence of two forms of the enzyme, one active and one non-active, is proposed. The natural variability of the PME activity was taken into the model in the form of normally distributed random effects. The common model parameters obtained (cleavage constant (0.0395±0.0062 s?1), degradation constant (0.556±0.112 s?1), cleavage energy of activation (469±23 kJ mol?1) and degradation energy of activation (488±18 kJ mol?1)) show that the PME degradation kinetics of the two vegetables can be explained with a single set of parameters. 相似文献
The reaction of Ru(XTPP)(DMF)2, where XTPP is the dianion of para substituted tetraphenylporphyrins and X is MeO, Me, H, Cl, Br, I, F, with O2 and CO were studied in DMF. The process was found to be first-order in metalloporphyrin, first-order in molecular oxygen and carbon monoxide, and second-order overall. Second-order rate constants for the CO reaction ranged from 0.170 to 0.665 M?1 s?1 at 25°C, those for the O2 reaction from 0.132 to 0.840 M?1 s?1 at 25°C. Similar activation parameters (ΔHCO± = 87 ± 1 kJ mol?1, ΔSCO± = 22 ± 4 JK?1 mol?1; ΔHO2± = 81 ± 1 kJ mol?1, and ΔSO2± = 11 ± 5 JK?1 mol?1) were found within each series. Reactivities of X substituted metalloporphyrins were found to follow different Hammett σ functions. The CO reactions correlated with σ? following normal behavior; the O2 reactions correlated with σ8° indicating O2 is π-bonded in the transition states. A dissociative mechanism is postulated for the process. 相似文献
AbstractThis research is focussed on kinetic, thermodynamic and thermal inactivation of a novel thermostable recombinant α-amylase (Tp-AmyS) from Thermotoga petrophila. The amylase gene was cloned in pHIS-parallel1 expression vector and overexpressed in Escherichia coli. The steady-state kinetic parameters (Vmax,Km, kcat and kcat/Km) for the hydrolysis of amylose (1.39?mg/min, 0.57?mg, 148.6?s?1, 260.7), amylopectin (2.3?mg/min, 1.09?mg, 247.1?s?1, 226.7), soluble starch (2.67?mg/min, 2.98?mg, 284.2?s?1, 95.4) and raw starch (2.1?mg/min, 3.6?mg, 224.7?s?1, 61.9) were determined. The activation energy (Ea), free energy (ΔG), enthalpy (ΔH) and entropy of activation (ΔS) at 98?°C were 42.9?kJ mol?1, 74?kJ mol?1, 39.9?kJ mol?1 and ?92.3 J mol?1 K?1, respectively, for soluble starch hydrolysis. While ΔG of substrate binding (ΔGE-S) and ΔG of transition state binding (ΔGE-T) were 3.38 and ?14.1?kJ mol?1, respectively. Whereas, EaD, Gibbs free energy (ΔG*), increase in the enthalpy (ΔH*) and activation entropy (ΔS*) for activation of the unfolding of transition state were 108, 107, 105?kJ mol?1 and ?4.1 J mol?1 K?1. The thermodynamics of irreversible thermal inactivation of Tp-AmyS revealed that at high temperature the process involves the aggregation of the protein. 相似文献
Decomposition of phenyl acridinium-9-carboxylate is monitored using electrogenerated chemiluminescence in a flow system. The formation of the pseudobase from the acridinium ester [AE] is described by rate = k′1[AE] + k″1[AE][OH?]0.5, where k′1 = 0.020 ± 0.006 s?1 and k″1 = 2.1 ± 0.8 (L/mol)?0.5 s?1. Irreversible decomposition of the pseudobase is described by rate = k′2[AE][OH?], where k′2 = 20.1 ± 3.8 (L/mol s). These kinetic equations, plus measurement of variation in emission intensity for constant acridinium ester concentration, are used to predict the resulting emission intensity v. pH behaviour given various contact times (in the 0.25 to 25 s range) for the acridinium ester to be in an alkaline solution prior to initiation of the chemiluminescence reaction. 相似文献
The rate constant, kd, for the dimerization of the free radical (NAD·), produced on the initial one-electron reduction of NAD+, was measured by double potential-step chronoamperometry, fast-scan cyclic voltammetry (cathodic-anodic peak current ratio) and slow-scan cyclic voltammetry (peak potential shift) for a medium in which neither NAD+ nor its reduction products are adsorbed at the solution/electrode interface. All three methods give concordant values of kd (approx. 3·107 M?1·s?1), which are in reasonable accord with the values determined by pulse radiolysis but are considerably greater than values previously determined electrochemically. For the NAD+/NAD· couple, the heterogeneous rate constant (ks,h) exceeds 1 cm·s?1 at 25°C and the formal potential (E0c) vs. sce is ? 1.155 V at 25°C and ? 1.149 V at 1°C at pH 9.1, with an uncertainty of about ±0.005 V. 相似文献
The kinetics of methemoglobin reduction by Fe(EDTA)2? have been studied and found to follow a second order rate law with k = 29.0 ?1 s?1 [25°C, μ = 0.2 , pH 7.0 (phosphate)], , and . The electrostatics-corrected self-exchange rate constant (k11corr) for hemoglobin based on the Fe(EDTA)2? cross-reaction is 2.79×10?3?1 s?1. This rate constant is compared with others reported for a water-soluble iron porphyrin and calculated from published data for the reactions of myoglobin and hemoglobin with Fe(EDTA)2? and Fe(CDTA)2?/?. The k11corr values for these systems range over ten orders of magnitude with heme ? myoglobin > hemoglobin. 相似文献
The sulfite radical anion (SO3?) is the first intermediate in the autoxidation of sulfite to sulfate. Using competition kinetics, its reactivities with the nucleic acid bases and the corresponding nucleosides were investigated. The second order rate constants were found to be rather low, k < 1 × 106dm3mol?1s?1 at pH 7. As a competitor, the carotenoid crocin was used, which was found to be bleached very efficiently by SO3? (k = 1.0 × 109dm3mol?1S?1). 相似文献
