Enhanced chemiluminescence in the oxidation of luminol and an isoluminol cortisol conjugate by hydrogen peroxide in reversed micelles

The chemiluminescent oxidation of luminol and an isoluminol cortisol conjugate (ABICOR) by hydrogen peroxide has been studied in cetyltrimethylammonium bromide (CTAB) reversed micelles in octane-chloroform (1 : 1). The maximum chemiluminescence intensity of both compounds is dependent on the initial concentrations of the H₂O₂ and substrates, the pH value of the micelle polar phase and the H₂O/CTAB ratio. The optimum pH ranged from 8.5 to 9.5. Under comparable conditions, the chemiluminescence intensity for luminol was 15-fold higher than for the ABI-COR conjugate. A mechanism of oxidation of the substrates in reversed micelles is proposed and the possible mechanisms of inhibition by the substrate and oxidant is discussed.     

Detection of hydrogen peroxide with chemiluminescent micelles

The overproduction of hydrogen peroxide is implicated in the progress of numerous life-threatening diseases and there is a great need for the development of contrast agents that can detect hydrogen peroxide in vivo. In this communication, we present a new contrast agent for hydrogen peroxide, termed peroxalate micelles, which detect hydrogen peroxide through chemiluminescence, and have the physical/chemical properties needed for in vivo imaging applications. The peroxalate micelles are composed of amphiphilic peroxalate based copolymers and the fluorescent dye rubrene, they have a ‘stealth’ polyethylene glycol (PEG) corona to evade macrophage phagocytosis, and a diameter of 33 nm to enhance extravasation into permeable tissues. The peroxalate micelles can detect nanomolar concentrations of hydrogen peroxide (>50 nM) and thus have the sensitivity needed to detect physiological concentrations of hydrogen peroxide. We anticipate numerous applications of the peroxalate micelles for in vivo imaging of hydrogen peroxide, given their high sensitivity, small size, and biocompatible PEG corona.     

Enhanced chemiluminescence of the fluorescein–KIO4 system by CdTe quantum dots for determination of catechol

In this paper, a novel chemiluminescence (CL) system was introduced based on the use of CdTe quantum dots (QDs) with the mixture solutions of fluorescein and potassium periodate (KIO₄) in alkaline medium. The CL signal of an ultra‐weak system was strongly enhanced in the presence of QDs. The application of CdTe QDs–fluorescein–KIO₄ system is reported for the first time. It was found that catechol had a diminishing effect on the CL reaction. Under optimal experimental conditions, CL intensity decreased linearly in a 1 to 100 μM catechol concentration range, with a 0.18 μM detection limit. A possible reaction mechanism was proposed according to the results of kinetic analyses, CL spectra, ultraviolet–visible and fluorescence spectra. The results pointed to an efficient energy transfer between the CL energy donor CdTe QDs and acceptor fluorescein. Finally, the CL method was successfully applied to the determination of catechol in environmental water samples.     

Oxidation of arachidonic acid in micelles by superoxide and hydrogen peroxide

Arachidonic acid was co-oxidized by xanthine oxidase. Both superoxide radical and hydrogen peroxide were required for oxidation, as shown by essentially complete inhibition caused by superoxide dismutase or by catalase. Pure arachidonate, free of lipid hydroperoxides, was susceptible to this co-oxidation, and the presence of lipid hydroperoxides did not accelerate the process. The role of trace metals was indicated by the stimulatory effect of EDTA-Fe and by the inhibitory effect of diethylenetriamine pentaacetate. Initiation of arachidonate co-oxidation was due to a potent oxidant generated by the interaction of H2O2 and O2- in the presence of Fe, rather than to either O2- or H2O2 per se. Hence, mannitol, a scavenger of OH ., but not of O2- or H2O2, also inhibited oxidation. Arachidonic acid autoxidation, a much slower process than xanthine oxidase co-oxidation, was barely detectable on the time scale of these observations. Unlike the co-oxidation, autoxidation was autocatalytic and therefore accelerated by hydroperoxide products. Marked quantitative differences in the distribution of isomeric hydroperoxide products of enzymic co-oxidation, as compared to the autoxidation, were noted and their significance was discussed.     

Quantification of hydrogen peroxide in plant extracts by the chemiluminescence reaction with luminol

The chemiluminescence of luminol (3-aminophthalhydrazide) with H₂O₂ has been used to quantify endogenous amounts of H₂O₂ in plant tissues. The reaction is linear over at least three orders of magnitude between 10^?5 and 10^?2M H₂O₂. Interference by coloured compounds in the crude extract is calibrated by a purification step with Dowex AG 1-X8. The extract is calibrated with an internal H₂O₂ standard, and the specificity verified by H₂O₂ purging with catalase. The minimum delectability for H₂O₂ of this assay is at least 1 ng, corresponding to 0.1–1 g fresh material. Data are presented for the levels of H₂O₂ in potatoes after treatment with oxygen and ethylene, in tomatoes before and after ripening and in untreated germinating castor beans as well as in beans treated with aminotriazol to inhibit catalase activity. Though data using the titanium test are generally confirmed, the method presented here has the advantage of higher sensitivity and specificity.     

Chemiluminescence intensities and spectra of luminol oxidation by sodium hypochlorite in the presence of hydrogen peroxide

Hydrogen peroxide amplifies the chemiluminescence in the oxidation of luminol by sodium hypochlorite. A linear relationship between concentration of hydrogen peroxide and light intensity was found in the concentration range 5 × 10^?8?7.5 × 10^?6 mol/l. At 7.5 × 10^?6 mol/l H₂O₂ the chemiluminescence is amplified 550—fold. The chemiluminescence spectra of these reactions have a wavelength maximum at 431 nm independent of the concentration of hydrogen peroxide. The results indicate that hydrogen peroxide is a necessary component in the chemiluminescent oxidation of the luminol by sodium hypochlorite.     

Amines for detection of dopamine by generation of hydrogen peroxide and peroxyoxalate chemiluminescence

A range of nitrogen-containing compounds (alkyl amines, piperazines, cyclohexylamines and nitrogen heterocyclics) were investigated for generation of hydrogen peroxide from dopamine and detection by peroxyoxalate chemiluminescence. Imidazole, ethyleneurea and allantoin among the nitrogen heterocyclic compounds tested generated hydrogen peroxide from dopamine following incubation at 60°C, pH 9.5–10.5, for 0–30 min. Imidazole was the most effective for generation of hydrogen peroxide, but imidazole derivatives with a primary amine side chain (histamine) or thiol (ethylenethiourea) were not effective. The presence of a ketone group (ethyleneurea, allantoin) did not hinder the reaction. Under optimal conditions (30 min incubation, 50 mmol/L imidazole) 10.5 nmol of dopamine could be detected. The cyclohexylamines tested produced low amounts of hydrogen peroxide (0.09–2.74% of light intensity with imidazole), and the piperazines and the alkyl amines tested produced no detectable hydrogen peroxide. Imidazole reacts with the phenolic groups of dopamine in a different manner from monoamine oxidase, and a reagent containing imidazole, ethyleneurea or allantoin was useful for non-enzymatic detection of dopamine by peroxyoxalate chemiluminescence.© John Wiley & Sons, Ltd.     

Electrogenerated chemiluminescence of Pb(II)-bromide complexes

The electrochemistry and electrogenerated chemiluminescence (ECL) of Pb₄Br₁₁ ³⁻ in acetonitrile solution is reported. Pb₄Br₁₁ ³⁻ is formed in situ by the reaction of lead(II) and bromide ions with ECL generated upon sweep to positive potentials using tri-n-propylamine (TPrA) as an oxidative-reductive coreactant. An ECL efficiency (φ_ecl) of 0.0079 was obtained compared to Ir(ppy)₃ (ppy=2-phenylpyridine; φ_ecl=1). The ECL intensity peaks at a potential corresponding to oxidation of TPrA and Pb₄Br₁₁ ³⁻ indicating that emission is from the lead-bromide cluster.     

Enhancing and inhibiting effects of benzenediols on chemiluminescence of a novel cyclometallated iridium(III) complex

A novel chemiluminescence (CL) system, including the cyclometallated iridium(III) complex {tris[1‐(2,6‐dimethylphenoxy)‐4‐(4‐chlorophenyl)phthalazine]iridium}, potassium permanganate and oxalic acid, is proposed for the determination of benzenediols. This method is based on the fact that hydroquinone and catechol exhibited an inhibiting effect, while resorcinol exhibited an enhancing effect on CL intensity. The optimum conditions for CL emission were investigated. Under optimal conditions, the detection limits of hydroquinone, catechol and resorcinol were 6.4 × 10^?8, 2.7 × 10^?9 and 8.1 × 10^?7 mol/L, respectively. The method has been successfully applied to the determination of benzenediols in different types of water sample. The luminophors of the CL systems were all identified as the metal–ligand charge‐transfer (MLCT) excited state of the iridium complex. Copyright © 2011 John Wiley & Sons, Ltd.     

Luminol-hydrogen peroxide chemiluminescence produced by sweet potato peroxidase.

Anionic sweet potato peroxidase (SPP; Ipomoea batatas) was shown to efficiently catalyse luminol oxidation by hydrogen peroxide, forming a long-term chemiluminescence (CL) signal. Like other anionic plant peroxidases, SPP is able to catalyse this enzymatic reaction efficiently in the absence of any enhancer. Maximum intensity produced in SPP-catalysed oxidation of luminol was detected at pH 7.8-7.9 to be lower than that characteristic of other peroxidases (8.4-8.6). Varying the concentrations of luminol, hydrogen peroxide and Tris buffer in the reaction medium, we determined favourable conditions for SPP catalysis (100 mmol/L Tris-HCl buffer, pH 7.8, containing 5 mmol/L hydrogen peroxide and 8 mmol/L luminol). The SPP detection limit in luminol oxidation was 1.0 x 10(-14) mol/L. High sensitivity in combination with the long-term CL signal and high stability is indicative of good promise for the application of SPP in CL enzyme immunoassay.     

Enhanced chemiluminescence of peroxomonosulfate–cobalt (II) system in the presence of dicarboxylic acids

In the present work, the effects of molecular mass aliphatic dicarboxylic acids on the HSO₅^‐–Co²⁺ chemiluminescence (CL) system were investigated. It was found that the aliphatic dicarboxylic acids could enhance the CL of the HSO₅^‐–Co²⁺ system. Moreover, the CL intensities improved regularly with increasing carbon chain length of the dicarboxylic acids. To investigate the CL enhancement mechanism, dynamic profiles, CL spectroscopy, ESR spectrum and the effects of various free radical scavengers on the CL system were employed. The results indicated that the enhancement of the CL should be attributed to the formation of peroxo‐diacid, which finally decomposed to the original dicarboxylic acid and singlet oxygen. The mechanism of the HSO₅^‐–Co²⁺‐dicarboxylic acid CL system was then proposed. Copyright © 2010 John Wiley & Sons, Ltd. Copyright © 2010 John Wiley & Sons, Ltd.     

Detection of lipid hydroperoxides and hydrogen peroxide at picamole levels by an HPLC and isoluminol chemiluminescence assay

An isoluminol assay is utilized for the detection. of hydrogen peroxide and lipid hydroperoxides in biological samples. The combination of this assay as a post-column detection for HPLC avoids interference of antioxidants and enables characterization of hydroperoxides at picomole levels. Two useful HPLC conditions for the separation of hydrogen peroxide, lipid hydroperoxides, antioxidants, and unoxidized lipids are described.     

Growth of Rhizobium sp. in the presence of catechol

The ability of Rhizobium sp., isolated from Lablab purpureus to survive in soil containing a phenolic derivative catechol was investigated. It survived for 9 months in soil containing catechol. In synthetic medium, Rhizobium sp. utilized catechol up to 10 mM as sole carbon source and catechol 1, 2-dioxygenase was present in the catechol grown cells. In the presence of organic acids and sugars, catechol was co-metabolized; but catechol 1, 2-dioxygenase induction was inhibited. The ability of Rhizobium sp. to utilize various phenolic substances provides potential advantage to overcome the phenolic toxicants present in soils.     

Metal-catalyzed oxidation of alpha-synuclein in the presence of Copper(II) and hydrogen peroxide

alpha-Synuclein is a component of abnormal protein depositions of Lewy bodies and senile plaques found in Parkinson's and Alzheimer's diseases, respectively. By using chemical coupling reagents such as dicyclohexylcarbodiimide or N-(ethoxycarbonyl)-2-ethoxy-1, 2-dihydroquinoline, the protein was shown to experience self-oligomerization in the presence of either copper(II) or Abeta25-35. The oligomers which appeared as a ladder on a 10-20% Tricine/SDS-PAGE have been suggested to participate in the formation of protein aggregations by possibly providing a nucleation center. Since oxidatively modified protein could increase its own tendency toward protein aggregation, metal-catalyzed oxidation of alpha-synuclein has been examined with copper(II) and hydrogen peroxide in the absence of the coupling reagent. Intriguingly, the protein was also self-oligomerized into an SDS-resistant ladder on the gel. This biochemically specific copper-mediated oxidative oligomerization was shown to be dependent upon the acidic C-terminus of alpha-synuclein because the C-terminally truncated proteins such as alpha-syn114 and alpha-syn97 were not affected by the metal and hydrogen peroxide. More importantly, the oxidative oligomerization was synergistically enhanced by the presence of Abeta25-35, indicating that the peptide interaction with alpha-synuclein facilitated the copper(II) binding to the acidic C-terminus and subsequent oxidative crosslinking. It has been, therefore, suggested that abnormalities in copper and H(2)O(2) homeostasis and certain pathological factors functionally similar to the Abeta25-35 could play critical roles in the metal-catalyzed oxidative oligomerization of alpha-synuclein, which may lead to possible protein aggregation and neurodegenerations.     

Electrogenerated chemiluminescence of (bis-bipyridyl)ruthenium(II) acetylacetonate complexes

The synthesis, electrochemistry, spectroscopy and electrogenerated chemiluminescence (ECL) of five bis-bipyridine ruthenium(II) complexes containing acetylacetonate complexes are reported. More specifically, (bpy)₂Ru(BA)₂(PF₆) (bpy = 2,2′-bipyridine; BA = benzoylacetonate), (bpy)₂Ru(TTFA)(PF₆) (TTFA =  thenoyltrifluoroacetonate), (bpy)₂Ru(TFPB)(PF₆) (TFPB = 4,4,4-trifluoro-1-phenyl-1,3-butanedionate), (bpy)₂Ru(TFPD)(PF₆) (TFPD =  1,1,1-trifluoro-2-4-pentanedionate), and (bpy)₂Ru(DBM)(PF₆) (DBM = dibenzoylmethide) display UV-Vis, photoluminescence, electrochemical and ECL properties characteristic of ruthenium bipyridyl complexes. All complexes display absorptions in the UV and visible regions of the spectra, with visible absorptions ranging from 350 to 700 nm, typical of metal-to-ligand charge transfer (MLCT) transitions. Photoluminescence emission maxima are also characteristic of MLCT transitions with wavelength maxima from 575 to 600 nm depending on the nature of the acetylacetonate ligand. ECL efficiencies for the complexes (?_ecl ∼ 0.013-0.051) are much lower than a standard (?_ecl = 1) with electron-withdrawing substituents resulting in lower efficiencies.     

Degradation of high-molecular-weight hyaluronan by hydrogen peroxide in the presence of cupric ions

Dynamic viscosity (eta) of the high-molecular-weight hyaluronan (HA) solution was measured by a Brookfield rotational viscometer equipped with a Teflon cup and spindle of coaxial cylindrical geometry. The decrease of eta of the HA solution, indicating degradation of the biopolymer, was induced by a system containing H2O2 alone or H2O2 plus CuCl2. The reaction system H2O2 plus CuCl2 as investigated by EPR spin-trapping technique revealed the formation of a four-line EPR signal characteristic of a *DMPO-OH spin adduct. Thus, hydroxyl radicals are implicated in degradation of high-molecular-weight HA by the system containing H2O2 and CuCl2.     

Copper(II) ethylenediaminetetraacetate complex does activate hydrogen peroxide in the presence of biological reductants.

The reaction of CuII (edta) (edta: ethylenediaminetetraacetic acid) with hydrogen peroxide (H2O2) was studied in the pH range of 6.0 to 8.0. CuII (edta) did not react with H2O2 in the all pH range examined in the absence of biological reductants. CuII (edta), however, could react with H2O2 in the presence of biological reductants such as ascorbic acid, cysteine and NADH to give thibarbituric acid (TBA) reactive substance, regardless of the pH. From these results, it is concluded that CuII (edta) cannot be bound to H2O2 and that the change of the redox potential of Cu2+ ion on ligating with edta may cause CuII (edta) to be unable to oxidize H2O2.     

Reaction mechanism of surfactant‐sensitized chemiluminescence of bis(2,4,6‐trichlorophyenyl) oxalate and hydrogen peroxide induced by gold nanoparticles

The chemiluminescence (CL) of bis(2,4,6‐trichlorophyenyl) oxalate with hydrogen peroxide in the present of cationic surfactant and gold nanoparticles was studied. The CL emission was obviously enhanced in the presence of surfactant at a suitable concentration, with a synergetic catalysis effect exhibited. Different sizes of gold nanoparticles (15 and 50 nm) showed different effects on CL intensity. Mechanisms of the CL reaction and sensitization effect are discussed. Copyright © 2008 John Wiley & Sons, Ltd.     

Detection of substances with alcoholic or phenolic hydroxyl groups by generation of hydrogen peroxide with imidazole and peroxyoxalate chemiluminescence

On-line detection of substances with an alcoholic or phenolic hydroxyl group using imidazole and peroxyoxalate chemiluminescence was investigated qualitatively using a flow-injection method. The substances tested included six polyphenols, five monophenols and six sugars. After incubation at 80°C with an imidazole buffer (pH 9.5) the substances were detected by peroxyoxalate chemiluminescence. The polyphenols tested (e.g., pyrogallol, purpurogallin, and dopamine) showed the strongest light emission. The sugars with hydroxyl groups (e.g., fructose and lactose) and the monophenols (e.g., phenol, serotonin, and β-estradiol) produced only a weak light emission. Reaction of hydroxyl compounds and imidazole generated hydrogen peroxide. Imidazole served two roles, it catalysed the reaction with the hydroxyl compound and initiated peroxyoxalate chemiluminescence on-line. A novel reactor formed by packing glass beads into a flow cell (Teflon) of a chemiluminometer improved the sensitivity of light detection.     

Photoluminescence and electrogenerated chemiluminescence of a bis(bipyridyl)ruthenium(II)-porphyrin complex

The photoluminescence (PL) and electrogenerated chemiluminescence (ECL) of [H₂(MPy3,4DMPP)Ru(bpy)₂Cl](PF₆), where H₂MPy3,4DMPP = meso-tris-3,4-dimethoxyphenyl-mono-(4-pyridyl)porphyrin and bpy = 2,2′-bipyridine, are reported in acetonitrile. The compound has a complex absorbance spectrum with bands characteristic of both the porphyrin and ruthenium moieties. PL emission maxim are observed at 655 nm when excited at the maximum absorption intensity corresponding to the porphyrin Soret π → π^∗ band, and around 600 nm when excited at wavelengths corresponding to Ru(dπ)-bpy (π^∗) MLCT transition. The photoluminescence efficiency (?_em) of the 655 nm emission is 0.039 and that of the free porphyrin is 0.69 compared to at 0.042.[H₂(MPy3,4DMPP)Ru(bpy)₂Cl](PF₆) displays complex electrochemical behavior, with one electrochemically reversible Ru^II-Ru^III oxidation and two quasi-reversible waves at more cathodic potentials corresponding to the porphyrin moiety. Oxidative ECL was generated using the coreactant tri-n-propylamine (TPrA). ECL efficiencies (?_ecl) were 0.14 for [H₂(MPy3,4DMPP)Ru(bpy)₂Cl]⁺ and 0.099 for H₂MPy3,4DMPP using as the standard (?_ecl = 1). ECL intensity was linear with respect to concentration from 1 to 0.001 μM.The ECL intensity peaks at potentials corresponding to oxidation both the ruthenium and porphyrin moieties as well as TPrA, indicating that multiple pathways for formation of the excited state are possible. However, an ECL spectrum shows a band similar in energy and shape to that of the Soret emission (655 nm for the PL and 656 nm for the ECL, respectively), indicating the same excited state is formed in each experiment.