Tyrosinase function

Pal et al. (1994) compared the catalysis of oxidative coupling reactions of various phenolic compounds by the enzymes, laccase and tyrosinase, and mineral catalyst, birnessite. Birnessite acts as a heterogeneous catalyst whereas laccase and tyrosinase function as homogeneous catalysts. Laccase and tyrosinase continue to oxidize catechol after repeated additions of the chemical, while birnessite lost its oxidizing activity after the first addition of catechol (Figure 2.20). In the case of birnessite,... 

Genetic disruption of dopamine synthesis in mice lacking TH shows that dopamine is not essential for development. However, dopamine deficient mice do not survive long after weaning unless treated with l-DOPA. These mice display severe aphagia and adipsia and loss of motor function. While these mice have a major reduction in dopamine levels some residual dopamine can be detected that is generated through the action of tyrosinases. 

The early works by Muzzarelh et al. [179] showed that tyrosinase converts a wide range of phenohc substrates into electrophihc o-quinones [180]. Tyrosinase was used to convert phenols into reactive o-quinones which then underwent chemical reactions leading to grafting onto chitosan. A review article showed that in general the tyrosinase-catalyzed chitosan modifications resulted in dramatic changes in functional properties [181]. 

Beermann, F., Ruppert, S., Hummler, E., Bosch, F. X., Muller, G., Riither, U., and Schiitz, G. (1990). Rescue of the albino phenotype by introduction of a functional tyrosinase gene into mice. EMBO J. 9 2819-2826. 

Muller, G Ruppert, S., Schmid, E and Schutz, G. (1988). Functional analysis of alternatively spliced tyrosinase gene transcripts. EMBO J. 7 2723-2730. 

In 1996, the first successful combination of an enzymatic with a nonenzymatic transformation within a domino process was reported by Waldmann and coworkers [6]. These authors described a reaction in which functionalized bicy-clo[2.2.2]octenediones were produced by a tyrosinase (from Agaricus bisporus) -catalyzed oxidation of para-substituted phenols, followed by a Diels-Alder reaction with an alkene or enol ether as dienophile. Hence, treatment of phenols such as 8-1 and an electron-rich alkene 8-4 in chloroform with tyrosinase in the presence of oxygen led to the bicyclic cycloadducts 8-5 and 8-6 in moderate to good yield (Scheme 8.1). It can be assumed that, in the first step, the phenol 8-1 is hydroxylated by tyrosinase, generating the catechol intermediate 8-2, which is then again oxidized enzy-... 

Some non-silica sol-gel materials have also been developed to immobilize bioactive molecules for the construction of biosensors and to synthesize new catalysts for the functional devices. Liu et al. [33] proved that alumina sol-gel was a suitable matrix to improve the immobilization of tyrosinase for detection of trace phenols. Titania is another kind of non-silica material easily obtained from the sol-gel process [34, 35], Luckarift et al. [36] introduced a new method for enzyme immobilization in a bio-mimetic silica support. In this biosilicification process precipitation was catalyzed by the R5 peptide, the repeat unit of the silaffin, which was identified from the diatom Cylindrotheca fusiformis. During the enzyme immobilization in biosilicification the reaction mixture consisted of silicic acid (hydrolyzed tetramethyl orthosilicate) and R5 peptide and enzyme. In the process of precipitation the reaction enzyme was entrapped and nm-sized biosilica-immobilized spheres were formed. Carturan et al. [11] developed a biosil method for the encapsulation of plant and animal cells. 

Adults require 1-2 mg of copper per day, and eliminate excess copper in bile and feces. Most plasma copper is present in ceruloplasmin. In Wilson s disease, the diminished availability of ceruloplasmin interferes with the function of enzymes that rely on ceruloplasmin as a copper donor (e.g. cytochrome oxidase, tyrosinase and superoxide dismutase). In addition, loss of copper-binding capacity in the serum leads to copper deposition in liver, brain and other organs, resulting in tissue damage. The mechanisms of toxicity are not fully understood, but may involve the formation of hydroxyl radicals via the Fenton reaction, which, in turn initiates a cascade of cellular cytotoxic events, including mitochondrial dysfunction, lipid peroxidation, disruption of calcium ion homeostasis, and cell death. 

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... 

Waldmann et al. used tyrosinase which is obtained from Agaricus bisporus for the oxidation of phenols to give ortho-quinones via the corresponding catechols in the presence of oxygen (scheme 33).1881 A combination of this enzymatic-initiated domino process with a Diels-Alder reaction yields the functionalized bicyclic components 164 and 165 as a 33 1 mixture starting from simple p-methyl-phenol 160 in the presence of ethyl vinyl ether 163 as an electron rich dienophile via the intermediates 161 and 162 in an overall yield of 77%. 

Our biomimetic investigations have focused on the metalloproteins hemocyanin (He) (11-17) and tyrosinase (11,12,14,16,18,29), which contain two copper ions in their active center. The function of hemocyanin is to bind and transport dioxygen in the hemolymph of molluscs and arthropods. Studies employing EXAFS spectroscopy have shown that in the deoxy form, two (19-21) or three (13,21) imidazole units fiom protein histidine residues coordinate to each cuprous ion. Upon addition of O2 to give oxy-Hc, considerable changes take place in the coordination sphere giving rise to tetragonally coordinated Cu(II) ions... 

Hemocyanin [30,31], tyrosinase [32] and catechol oxidase (2) [33] comprise this class of proteins. Their active sites are very similar and contain a dicopper core in which both Cu ions are ligated by three N-bound histidine residues. All three proteins are capable of binding dioxygen reversibly at ambient conditions. However, whereas hemocyanin is responsible for O2 transport in certain mollusks and arthropods, catechol oxidase and tyrosinase are enzymes that have vital catalytic functions in a variety of natural systems, namely the oxidation of phenolic substrates to catechols (Scheme 1) (tyrosinase) and the oxidation of catechols to o-quinones (tyrosinase and catechol oxidase). Antiferromagnetic coupling of the two Cu ions in the oxy state of these metalloproteins leads to ESR-silent behavior. Structural insight from X-ray crystallography is now available for all three enzymes, but details... 

Fukuzumi and Itoh have jointly reported on a if-peroxo dicop-per(ll) complex that acts as a functional model for the phenolase activity of tyrosinase. lithium salts of para-substituted phenols were used as substrates, reaching yields between 60 and 90% with only the catechol product formed... 

Fukuzumi and co-workers described spectroscopic evidence for a ix-rf- ] -peroxo-(Cu )2 species stabilized with a fcidentate nitrogen ligand, but no (catalytic) oxidation behavior towards catechol was noted (a related trinu-clear copper species converted 2,4-di-ferf-butylphenol stoichiometrically towards the biphenol derivative) [224], Stack et al. have described a similar ] -peroxo-(Cu )2 species (28, vide supra) that could be considered a structural and functional model for tyrosinase-activity, as it efficiently reacted with catechol, benzyl alcohol and benzylamine to yield quinone (95%), benzaldehyde (80%) and benzonitrile (70%) [172,173]. This dinuclear per-0X0 species is generated by association of two monomeric copper centers, in contrast to the systems based on dinucleating Ugand scaffolds described above. 

Tyrosinase is both an oxidase and a hydroxylase. Some other copper enzymes have only a hydroxylase function. One of the best understood of these is the peptidylglycine a-hydroxylating monoxygenase, which catalyzes the first step of the reaction of Eq. 10-11. The enzyme is a colorless two-copper protein but the copper atoms are 1.1 nm apart and do not form a binuclear center.570 Ascorbate is an essential cosubstrate, with two molecules being oxidized to the semidehydro-ascorbate radical as both coppers are reduced to Cu(I). A ternary complex of reduced enzyme, peptide, and 02 is formed and reacts to give the hydroxylated product.570 A related two-copper enzyme is dopamine (J-monooxygenase, which utilizes 02 and ascorbate to hydroxylate dopamine to noradrenaline (Chapter 25).571/572 These and other types of hydroxylases are compared in Chapter 18. 

Figure 2.22. Initial velocity of oxygen consumption as a function of the substrate (catechol) concentration in the presence of 0.074mg (7.11 x 1(T9M) tyrosinase (A), 2.0mg (2.8 x 1(T4M with a corresponding concentration of the mineral active sites, [M5]1.71xl(r6) of 8-Mn02 (B) and 10.0 mg (1.40 x 10 3M with a corresponding concentration of the mineral active sites, [M ]8.54 x 10-6) of S-Mn02 (C). Reprinted from Naidja, A., Liu, C., and Huang, P. M. (2002). Formation of protein-birnessite complex XRD, FTIR, and AFM analysis. J. Coll. Interface Sci. 251,46-56, with permission from Elsevier.

As the focus of this review is on copper-dioxygen chemistry, we shall briefly summarize major aspects of the active site chemistry of those proteins involved in 02 processing. The active site structure and chemistry of hemocyanin (He, 02 carrier) and tyrosinase (Tyr, monooxygenase) will be emphasized, since the chemical studies described herein are most relevant to their function. The major classes of these proteins and their origins, primary functions, and leading references are provided in Table 1. Other classes of copper proteins not included here are blue electron carriers [13], copper-thiolate proteins (metallothioneines) [17], and NO reductases (e.g., nitrite [NIR] [18] or nitrous oxide [19]). 

Tyrosine, itself a degradation product of phenylalanine (Sec. 15.1), is initially converted to 3.4-dihydroxyphenylalanine (dopa), and the corresponding do pa quinone, by the copper-containing enzyme tyrosinase. Tyrosinase is found in melanocytes and is a mixed-function oxidase. It catalyzes the following reaction ... 

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