Oxidases ascorbate

Enzymes often need for their activity the presence of a non-protein portion, which may be closely combined with the protein, in which case it is called a prosthetic group, or more loosely associated, in which case it is a coenzyme. Certain metals may be combined with the enzyme such as copper in ascorbic oxidase and selenium in glutathione peroxidase. Often the presence of other metals in solution, such as magnesium, are necessary for the action of particular enzymes. 

Another approach to improve selectivity is to use an enzyme electrode. The enzyme ascorbate oxidase has been used successfully to remove ascorbate as an interference of in vivo voltammetric electrodes 219,320) Ascorbate oxidase converts the ascorbic acid to dehydroascorbate which is not electroactive in the potential region used for in vivo analysis. 

Blake, D.R., Blann( A., Bacon, P.A., Farr, M., Gutteridge, J.M.C. and Halliwell, B. (1983). Ferroxidase and ascorbate oxidase activities in synovial fluid from rheumatoid joints. Clin. Sci. 64, 551-553. 

Figure 12.1 Structure of the four copper sites in ascorbate oxidase showing their spatial relationship. From Lippard and Berg, 1994. Reproduced by permission of University Science Books.

Nitric oxide reductase (P) Nitrous oxide reductase (P) Ascorbate oxidase (P) Cytochrome oxidase (PM) Copper ATPase pumps (PM)... 

Many multiple copper containing proteins (e.g., laccase, ascorbate oxidase, hemo-cyanin, tyrosinase) contain so-called type III copper centers, which is a historical name (cf. Section 5.8 for type I and type II copper) for strongly exchange-coupled Cu(II) dimers. In sharp contrast to the ease with which 5=1 spectra from copper acetate are obtained, half a century of EPR studies on biological type III copper has not produced a single triplet spectrum. Why all type III centers have thus far remained EPR silent is not understood. 

K. Rekha, M.D. Gouda, M.S. Thakur, and N.G. Karanth, Ascorbate oxidase based amperometric biosensor for organophosphorous pesticide monitoring. Biosens. Bioelectron. 15, 499-520 (2000). 

Catalytic reduction of oxygen directly to water, while not as yet possible with traditional catalyst technology at neutral pH, is achieved with some biocatalysts, particularly by enzymes with multi-copper active sites such as the laccases, ceruloplasmins, ascorbate oxidase and bilirubin oxidases. The first report on the use of a biocatalyst... 

Under stress conditions, such as cutting or light exposure, ascorbate oxidase has been described as promoting the transformation of ascorbic acid to dehydroascorbic acid (Wright and Kader 1997b). However, because ascorbic acid can be easily converted into dehydroascorbic acid, it is necessary to measure both ascorbic and dehydroascorbic acids to observe that the content of vitamin C was well preserved in fresh-cut fruit. 

Various spectroscopic methods have been used to probe the nature of the copper centers in the members of the blue copper oxidase family of proteins (e.g. see ref. 13). Prior to the X-ray determination of the structure of ascorbate oxidase in 1989, similarities in the EPR and UV-vis absorption spectra for the blue multi-copper oxidases including laccase and ceruloplasmin had been observed [14] and a number of general conclusions made for the copper centers in ceruloplasmin as shown in Table 1 [13,15]. It was known that six copper atoms were nondialyzable and not available to chelation directly by dithiocarbamate and these coppers were assumed to be tightly bound and/or buried in the protein. Two of the coppers have absorbance maxima around 610 nm and these were interpreted as blue type I coppers with cysteine and histidine ligands, and responsible for the pronounced color of the protein. However, they are not equivalent and one of them, thought to be involved in enzymatic activity, is reduced and reoxidized at a faster rate than the second (e.g. see ref. 16). There was general concurrence that there are two type HI... 

Ceruloplasmin is a member of the family of blue copper oxidases which also contains laccase and ascorbate oxidase. The relationship... 

Figure 6. Structural relationships between ascorbate oxidase, ceruloplasmin, nitrite reductase, and blood clotting factor VIII.

S / V CONTENTS Preface, Robert W. Hay. Structure and Function of Manganese-Containing Biomolecules, David C. Weather-bum. Repertories of Metal Ions as Lewis Acid Catalysts in Organic Reactions, Junghan Suh. The Multicopper-Enzyme Ascorbate Oxidase, Albrecht Messerschmidt. The Bioinorganic Chemistry of Aluminum, Tomas Kiss and Etelka Farkas. The Role of Nitric Oxide in Animal Physiology, Anthony R. Butler, Frederick Flitney and Peter Rhodes. Index. 

Type II copper enzymes generally have more positive reduction potentials, weaker electronic absorption signals, and larger EPR hyperfine coupling constants. They adopt trigonal, square-planar, five-coordinate, or tetragonally distorted octahedral geometries. Usually, type II copper enzymes are involved in catalytic oxidations of substrate molecules and may be found in combination with both Type I and Type III copper centers. Laccase and ascorbate oxidase are typical examples. Information on these enzymes is found in Tables 5.1, 5.2, and 5.3. Superoxide dismutase, discussed in more detail below, contains a lone Type II copper center in each of two subunits of its quaternary structure. 

Copper oxidases Blue oxidases (multicopper oxidases) Laccase Ascorbate oxidase Ceruloplasmin... 

Table 5.2 contains data about selected copper enzymes from the references noted. It should be understood that enzymes from different sources—that is, azurin from Alcaligenes denitrificans versus Pseudomonas aeruginosa, fungal versus tree laccase, or arthropodan versus molluscan hemocyanin—will differ from each other to various degrees. Azurins have similar tertiary structures—in contrast to arthropodan and molluscan hemocyanins, whose tertiary and quaternary structures show large deviations. Most copper enzymes contain one type of copper center, but laccase, ascorbate oxidase, and ceruloplasmin contain Type I, Type II, and Type III centers. For a more complete and specific listing of copper enzyme properties, see, for instance, the review article by Solomon et al.4... 

This discussion of copper-containing enzymes has focused on structure and function information for Type I blue copper proteins azurin and plastocyanin, Type III hemocyanin, and Type II superoxide dismutase s structure and mechanism of activity. Information on spectral properties for some metalloproteins and their model compounds has been included in Tables 5.2, 5.3, and 5.7. One model system for Type I copper proteins39 and one for Type II centers40 have been discussed. Many others can be found in the literature. A more complete discussion, including mechanistic detail, about hemocyanin and tyrosinase model systems has been included. Models for the blue copper oxidases laccase and ascorbate oxidases have not been discussed. Students are referred to the references listed in the reference section for discussion of some other model systems. Many more are to be found in literature searches.50... 

Copper oxidases are widely distributed in nature, and enzymes from plants, microbes, and mammals have been characterized (104,105). The blue copper oxidases, which include laccases, ascorbate oxidases, and ceruloplasmin, are of particular interest in alkaloid transformations. The principle differences in specificity of these copper oxidases are due to the protein structures as well as to the distribution and environment of copper(II) ions within the enzymes (106). While an in vivo role in metabolism of alkaloids has not been established for these enzymes, copper oxidases have been used in vitro for various alkaloid transformations. 

L-ascorbic acid Potentiometric Based on ascorbate oxidase of natural source immobilised on ethylene-vinylacetate membrane Fernandes et al. (1999)... 

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