Peroxidase oxygenations

Pancreatic ribonuclease Staphylococcal nuclease Peroxidases Glutathione peroxidase Cytochrome c peroxidase Oxygen carriers Myoglobin, hemoglobin Myohemerythrin, hemerythrin Hormone-binding proteins Uteroglobin Pre albumin Lectins... 

Peroxidase Oxygenations. Two poorly defined reactions are believed to represent a third type of oxygenation. In one, a well-defined enzyme, horseradish peroxidase (- -Mn++) appears to add molecular oxygen to substrates including dihydroxyfumarate and indoleacetate. The products are not weU-defined in this case. Another enzyme, tryptophan peroxidase, has not been purified sufficiently to permit its chemical nature to be ascertained. This enzyme carries out the stoichiometric conversion of tryptophan to formylkynurenine, with the addition of... 

Chemiluminescent Immunoassay. Chemiluminescence is the emission of visible light resulting from a chemical reaction. The majority of such reactions are oxidations, using oxygen or peroxides, and among the first chemicals studied for chemiluminescence were luminol (5-amino-2,3-dihydro-l,4-phthalazinedione [521-31-3]) and its derivatives (see Luminescent materials, chemiluminescence). Luminol or isoluminol can be directly linked to antibodies and used in a system with peroxidase to detect specific antigens. One of the first appHcations of this approach was for the detection of biotin (31). 

N—Fe(IV)Por complexes. Oxo iron(IV) porphyrin cation radical complexes, [O—Fe(IV)Por ], are important intermediates in oxygen atom transfer reactions. Compound I of the enzymes catalase and peroxidase have this formulation, as does the active intermediate in the catalytic cycle of cytochrome P Q. Similar intermediates are invoked in the extensively investigated hydroxylations and epoxidations of hydrocarbon substrates cataly2ed by iron porphyrins in the presence of such oxidizing agents as iodosylbenzene, NaOCl, peroxides, and air. 

Reaction takes place ia aqueous solution with hydrogen peroxide and catalysts such as Cu(II), Cr(III), Co(II), ferricyanide, hernia, or peroxidase. Chemiluminescent reaction also takes place with oxygen and a strong base ia a dipolar aprotic solvent such as dimethyl sulfoxide. Under both conditions Qcis about 1% (light emission, 375—500 am) (105,107). 

Catalytic oxidation of isobutyraldehyde with air at 30—50°C gives isobutyric acid [79-31-2] ia 95% yield (5). Certain enzymes, such as horseradish peroxidase, cataly2e the reaction of isobutyraldehyde with molecular oxygen to form triplet-state acetone and formic acid with simultaneous chemiluminescence (6). 

DET calculations on the hyperfine coupling constants of ethyl imidazole as a model for histidine support experimental results that the preferred histidine radical is formed by OH addition at the C5 position [00JPC(A)9144]. The reaction mechanism of compound I formation in heme peroxidases has been investigated at the B3-LYP level [99JA10178]. The reaction starts with a proton transfer from the peroxide to the distal histidine and a subsequent proton back donation from the histidine to the second oxygen of the peroxide (Scheme 8). 

Luminescence reaction. Pholasin undergoes an oxidative luminescence reaction in the presence of any of the following substances Pholas luciferase, ferrous ions, H2O2, peroxidases, superoxide anions, hypochlorite and other oxidants. In all cases, molecular oxygen is required and pholasin is converted into oxypholasin in the reaction. 

Two main groups can be discerned (1) endogenous factors such as plant enzymes like polyphenoloxidase, peroxidase, and P-glucosidase and (2) conditions prevailing in the extraction medium will decide the fates of betalain pigments among which temperature, oxygen, and pH are considered the most important conditions. 

Li D, M Alic, JA Brown, MH Gold (1995) Regulation of manganese peroxidase gene transcription by hydrogen peroxide, chemical stress, and molecular oxygen. Appl Environ Microbiol 61 341-345. 

Glutathione-peroxidase (GSH-Pxase) is an enzyme found in erythroqrtes and other tissues that has an essential selenocysteine residue involved in the catalytic decomposition of reactive oxygen species. In the erythrocyte, hydrogen peroxide is the principle reactive oxygen species available. 

Free radicals are by-products of prostaglandin metabolism and may even regulate the activity of the arachidonate pathway. Arachidonic acid, released from lipids as a result of activation of phospholipases by tissue injury or by hormones, may be metabolized by the prostaglandin or leu-kotriene pathways. The peroxidase-catalysed conversion of prostaglandin G2 to prostaglandin H2 (unstable prostanoids) and the mechanism of hydroperoxy fatty acid to the hydroxy fatty acid conversion both yield oxygen radicals, which can be detected by e.s.r. (Rice-Evans et al., 1991). 

Selenium is required, but levels must fall into a narrow window. Both deficiency and toxicity symptoms occur. The element is also used therapeutically in cancer treatment. It is the co-factor of the enzyme glutathione peroxidase which is thought to play an important role in oxygen toxicity. The determination of Se in blood or serum is not easy, as many incorrect, inaccurate and imprecise methods have been published (Magee and James 1994). A suggested procedure for Se in body fluids is based on GF-AAS (Thomassen et al. 1994)- For tissues SS-AAS may be used (Fler-ber 1994a). Recent developments by Turner et al. (1999) show that LC-ICP-MS is sensitive and reproducible at low levels. 

Black tea quality as determined by theaflavin levels is also affected by storage conditions. Low temperatures, low moisture levels, and low oxygen availability retard theaflavin loss. Residual peroxidase activity, which accelerates theaflavin loss on storage, is diminished by acid treatment during fermentation.94... 

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