32 research outputs found
Tryptophan-Accelerated Electron Flow Across a Protein−Protein Interface
We report a new metallolabeled blue copper protein, Re126W122Cu^I Pseudomonas aeruginosa azurin, which has three redox sites at well-defined distances in the protein fold: Re^I(CO)_3(4,7-dimethyl-1,10-phenanthroline) covalently bound at H126, a Cu center, and an indole side chain W122 situated between the Re and Cu sites (Re-W122(indole) = 13.1 Å, dmp-W122(indole) = 10.0 Å, Re-Cu = 25.6 Å). Near-UV excitation of the Re chromophore leads to prompt Cu^I oxidation (<50 ns), followed by slow back ET to regenerate Cu^I and ground-state Re^I with biexponential kinetics, 220 ns and 6 μs. From spectroscopic measurements of kinetics and relative ET yields at different concentrations, it is likely that the photoinduced ET reactions occur in protein dimers, (Re126W122CuI)2 and that the forward ET is accelerated by intermolecular electron hopping through the interfacial tryptophan: ^*Re//←W122←Cu^I, where // denotes a protein–protein interface. Solution mass spectrometry confirms a broad oligomer distribution with prevalent monomers and dimers, and the crystal structure of the Cu^(II) form shows two Re126W122Cu^(II) molecules oriented such that redox cofactors Re(dmp) and W122-indole on different protein molecules are located at the interface at much shorter intermolecular distances (Re-W122(indole) = 6.9 Å, dmp-W122(indole) = 3.5 Å, and Re-Cu = 14.0 Å) than within single protein folds. Whereas forward ET is accelerated by hopping through W122, BET is retarded by a space jump at the interface that lacks specific interactions or water molecules. These findings on interfacial electron hopping in (Re126W122Cu^I)^2 shed new light on optimal redox-unit placements required for functional long-range charge separation in protein complexes
The oxidation of luteolin, the natural flavonoid dye
The oxidation of natural flavonoid luteolin in aqueous solution is studied by electrochemical methods,
electron paramagnetic resonance (EPR), spectroelectrochemistry and separation techniques HPLC-DAD
and HPLC–MS/MS. The number of electrons involved in the oxidation of luteolin depends on the presence
of its dissociation forms in solution. The study explains the differences in the number of electrons
presented in the literature. The overall one electron oxidation mechanism of luteolin in alkaline solution
is explained by the comproportionation reaction of resulting quinone, despite the fact that quinone
is formed by two electron oxidation. Then a hydroxylation takes place. The EPR spectroelectrochemical
study of the semiquinone radical anion formation as well as of the reaction steps following the
electron transfer during the oxidation is presented. The novelty of this contribution consists in the additional
temperature controlled semi-quantitative in situ EPR spectroelectrochemical experiment of the
flavonoid oxidation. The data acquired by temperature controlled in situ EPR spectroelectrochemistry
supports the comproportionation/disproportionation equilibria as well as the oxidative decomposition
of luteolin and shows that the formation of a pi-dimer is less probable. The oxidation products hydroxyluteolin
and 3,5-dihydroxy-2-(2-oxoacetyl)phenyl-3,4-dihydroxybenzoate are not stable under ambient
conditions and decompose to low molecular hydroxycompounds such as 3,4-dihydroxybenzoic acid and
2,5,7-trihydroxy-4H-1-benzopyran-4-one
The oxidation of natural flavonoid quercetin
This study explains the controversies in the literature concerning
the number of electrons involved in the oxidation of quercetin.
This stems from inappropriate handling samples, which require
strict anaerobic conditions. The redox potential of quercetin
strongly depends on the pH and on the presence of dissociation
forms in solution
On the stability of the bioactive flavonoids quercetin and luteolin under oxygen-free conditions
The natural flavonoid compounds quercetin (3,3',4',5,7-pentahydroxyflavone) and luteolin (3',4',5,7-tetrahydroxyflavone) are important bioactive compounds with antioxidative, anti-allergic, and anti-inflammatory properties. However, both are unstable when exposed to atmospheric oxygen, which causes degradation and complicates their analytical determinations. The oxidative change of these flavonoids was observed and followed by UV-visible spectrophotometry, both in aqueous and ethanolic solutions. The distribution of the degradation products in aqueous media was monitored by LC-MS and LC-DAD analysis. The amounts of oxidative reaction products increase with the exposure time. The oxidative degradation reduces the pharmacological efficiency of these antioxidants and renders analytical determination inaccurate. The oxidative changes in flavonoid test solutions can explain the inconsistent dissociation constants reported in the literature. Dissociation constants of quercetin and luteolin were determined both by alkalimetric titration and by UV-visible spectrophotometry under deaerated conditions. The values pK (1) = 5.87 +/- 0.14 and pK (2) = 8.48 +/- 0.09 for quercetin, and pK (1) = 5.99 +/- 0.32 and pK (2) = 8.40 +/- 0.42 for luteolin were found
Cystathionine β‐synthase deficiency in the E‐HOD registry‐part I: pyridoxine responsiveness as a determinant of biochemical and clinical phenotype at diagnosis
Cystathionine β‐synthase (CBS) deficiency has a wide clinical spectrum, ranging from neurodevelopmental problems, lens dislocation and marfanoid features in early childhood to adult onset disease with predominantly thromboembolic complications. We have analysed clinical and laboratory data at the time of diagnosis in 328 patients with CBS deficiency from the E‐HOD (European network and registry for Homocystinurias and methylation Defects) registry. We developed comprehensive criteria to classify patients into four groups of pyridoxine responsivity: non‐responders (NR), partial, full and extreme responders (PR, FR and ER, respectively). All groups showed overlapping concentrations of plasma total homocysteine while pyridoxine responsiveness inversely correlated with plasma/serum methionine concentrations. The FR and ER groups had a later age of onset and diagnosis and a longer diagnostic delay than NR and PR patients. Lens dislocation was common in all groups except ER but the age of dislocation increased with increasing responsiveness. Developmental delay was commonest in the NR group while no ER patient had cognitive impairment. Thromboembolism was the commonest presenting feature in ER patients, whereas it was least likely at presentation in the NR group. This probably is due to the differences in ages at presentation: all groups had a similar number of thromboembolic events per 1000 patient‐years. Clinical severity of CBS deficiency depends on the degree of pyridoxine responsiveness. Therefore, a standardised pyridoxine‐responsiveness test in newly diagnosed patients and a critical review of previous assessments is indispensable to ensure adequate therapy and to prevent or reduce long‐term complications
Electrochemistry and spectroelectrochemistry of bioactive hydroxyquinolines: a mechanistic study
The oxidation mechanism of selected hydroxyquinoline carboxylic acids such as 8-hydroxyquinoline-7-carboxylic acid (1), the two positional isomers 2-methyl-8-hydroxyquinoline-7-carboxylic acid (3) and 2-methyl-5-hydroxyquinoline-6-carboxylic acid (4), as well as other hydroxyquinolines were studied in aprotic environment using cyclic voltammetry, controlled potential electrolysis, in situ UV vis and IR spectroelectrochemistry, and HPLC-MS/MS techniques. IR spectroelectrochemistry showed that oxidation unexpectedly proceeds together with protonation of the starting compound. We proved that the nitrogen atom in the heterocycle of hydroxyquinolines is protonated during the apparent 0.7 electron oxidation process. This was rationalized by the autodeprotonation reaction by another two starting molecules of hydroxyquinoline, so that the overall oxidation mechanism involves two electrons and three starting molecules. Both the electrochemical and spectroelectrochemical results showed that the oxidation mechanism is not influenced by the presence of the carboxylic group in the chemical structure of hydroxyquinolines, as results from oxidation of 2,7-dimethyl-S-hydroxyquinoline (6). In the presence of a strong proton acceptor such as pyridine, the oxidation ECEC process involves two electrons and two protons per one molecule of the hydroxyquinoline derivative. The electron transfer efficiency of hydroxyquinolines in biosystems may be related to protonation of biocompounds containing nitrogen bases. Molecular orbital calculations support the experimental findings
Application of spectroelectrochemistry in elucidation of electrochemical mechanism of azoquinoline dye 2-methyl-5-[(E)-phenyldiazenyl]quinolin-8-ol
In situ spectroelectrochemical detection of reaction intermediates was used as a decisive method for elucidation of a rather complex redox mechanism of azoquinoline dye 2-methyl-5-[(E)-phenyldiazenyl]quinolin-8-ol (R-N=N-Ph; where Ph = phenyl, R = 2-methyl-8-hydroxyquinoline fragment). Electrochemical properties were studied in non-aqueous solution by cyclic voltammetry, UV–Vis and IR spectroelectrochemistry and high pressure liquid chromatography with diode array detector. Oxidation and reduction mechanisms involve coupled electron and proton transfers. Oxidation proceeds primarily on hydroxyl group at quinoline moiety and (E)-5-(phenyldiazenyl)quinoline-7,8-diol as the main oxidation product has been suggested. The electrochemically active site for reduction is the azo group. This was proved by in situ UV–Vis and IR spectroelectrochemical data. Detailed analysis of the effects of the presence of acids and bases evidenced the presence of two species in equilibrium: HOR(NH+)-N=N-Ph and HOR-N=N-Ph. The compound containing the hydrazo group (5-(2-phenylhydrazinyl)quinolin-8-ol (R-N=N-Ph) is the main reduction product. Molecular orbital calculations and DFT calculations of IR spectra support the experimental results. In situ IR spectroelectrochemical experiments proved that no reaction of R-N=N-Ph anion or dianion with the solvent acetonitrile was observed during the reduction of the azodye
The oxidation mechanism of the antioxidant quercetin in nonaqueous media
The knowledge of the degradation pathways of natural dyes used in medieval textiles is necessary for the restoration of their original color. Quercetin, one of such colorants, reportedly yields the wide spectrum of oxidation products in different types of media. This study deals with electrochemical oxidation mechanism of quercetin in nonaqueous solution, which has not been yet attempted. The final oxidation product at the first oxidation wave was identified by HPLC-DAD and GC-MS techniques as 2-(3',4'-dihydroxybenzoyl)-2,4,6-trihydroxybenzofuran-3(2H)-one. The apparent two-electron process at the potential of the first oxidation wave yields current-voltage shapes with one-electron characteristics. The in situ spectroelectrochemistry measurements proved the oxidation mechanism leading through a short-lived anion radical. Two possibilities of the oxidation mechanism are discussed: two one-electron transfers, which do not have identical but similar redox potentials. or the presence of a disproportionation chemical reaction following the first one electron transfer. The quinone formed in either case is stable only on the time scale of a fast spectroelectrochemistry and undergoes fast hydroxylation reaction, where 2-(3,4-dihydroxybenzoyl)-2,4,6-trihydroxybenzofuran-3-one is formed. This compound is oxidized at the potential of the second oxidation wave of quercetin
The Role of Social Networks in Online Marketing and Measurement of Their Effectiveness – The Case Study
International audienceThis paper is devoted to online marketing tools and primarily focuses on the use of social networks and measuring their effectiveness. The theoretical part briefly presents the topic of online marketing and selected tools. The next section deals with the case study that analyses the use of social networks on a particular project, including measuring the efficiency of social networks by comparing the planned and actual state according to the selected metrics. In conclusion, there is a discussion on the results obtained and the possible directions, which would increase the efficiency of social networks, i.e. online marketing, are outlined. The results of assessing the current state of online marketing for the surveyed project in 2017, by comparing the planned and actual metric values, largely fail to meet the targets. With measuring social networking tools, the planned numbers of website visits and social networking orders didn’t reach their planned values. Regarding the number of fans on individual social networks, the planned status was only achieved with the Pinterest and Instagram social networks