Blue copper proteins function

We have used a range of different physical and chemical approaches in the effort to better understand how the different blue copper proteins function. With the relatively simpler, electron-mediating proteins like azurin, the ultraviolet chromophores were shown to be informative in terms of copper-protein interactions. These proteins are also a useful system for detailed examination of the electron transfer pathways to and from their single copper site. 

The many redox reactions that take place within a cell make use of metalloproteins with a wide range of electron transfer potentials. To name just a few of their functions, these proteins play key roles in respiration, photosynthesis, and nitrogen fixation. Some of them simply shuttle electrons to or from enzymes that require electron transfer as part of their catalytic activity. In many other cases, a complex enzyme may incorporate its own electron transfer centers. There are three general categories of transition metal redox centers cytochromes, blue copper proteins, and iron-sulfur proteins. 

Blue copper proteins. A typical blue copper redox protein contains a single copper atom in a distorted tetrahedral environment. Copper performs the redox function of the protein by cycling between Cu and Cu. Usually the metal binds to two N atoms and two S atoms through a methionine, a cysteine, and two histidines. An example is plastocyanin, shown in Figure 20-29Z>. As their name implies, these molecules have a beautiful deep blue color that is attributed to photon-induced charge transfer from the sulfur atom of cysteine to the copper cation center. 

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... 

Most mechanisms which control biological functions, such as cell respiration and photosynthesis (already discussed in Chapter 5, Section 3.1), are based on redox processes. In particular, as shown again in Figure 1, it is evident that, based on their physiological redox potentials, in photosynthesis a chain of electron carriers (e.g. iron-sulfur proteins, cytochromes and blue copper proteins) provides a means of electron transport which is triggered by the absorption of light. 

Blue copper proteins, 36 323, 377-378, see also Azurin Plastocyanin active site protonations, 36 396-398 charge, 36 398-401 classification, 36 378-379 comparison with rubredoxin, 36 404 coordinated amino acid spacing, 36 399 cucumber basic protein, 36 390 electron transfer routes, 36 403-404 electron transport, 36 378 EXAFS studies, 36 390-391 functional role, 36 382-383 occurrence, 36 379-382 properties, 36 380 pseudoazurin, 36 389-390 reduction potentials, 36 393-396 self-exchange rate constants, 36 401-403 UV-VIS spectra, 36 391-393 Blue species... 

Blue copper proteins are a family of metalloproteins that have been found to play an important role in a number of electron-transfer reactions in nature. Solomon and coworkers have studied a range of blue copper enzymes in detail to produce a thorough description of how molecular and electronic structure interact to provide the function of these enzymes (26,158). 

Porterfield. W. W., 295 Positive oxidation states, halogens in, 837-848 Posttransition metals, 28. 876 Potassium, 309, 582-587 Potentials, electrode, 378-383 Pourbaix diagram, 591-592 Praseo complex, 388,491, 493 Predominance area diagram, 591 Prewitt, C. T., 116-117 Principal axis, 51 Prism, trigonal prism, 489-491 Probability function, 13 Prosthetic group, 919 Proteins, and blue copper proteins, 912-916 Proton... 

Cytochromes c, small blue-copper proteins, or an internal heme c group can function as natural electron acceptors for the dehydrogenases. Since these are soluble proteins and the genes have been cloned in most cases, they provide excellent possibilities to study electron transfer pathways in vitro and intermolecular as well as intramolecular pathways between a quinone and Cu or heme c in particular. 

Copper proteins are involved in a variety of biological functions, including electron transport, copper storage and many oxidase activities. A variety of reviews on this topic are available (Sykes, 1985 Chapman, 1991). Several copper proteins are easily identified by their beautiful blue colour and have been labelled blue copper proteins. The blue copper proteins can be divided into two classes, the oxidases (laccase, ascorbate oxidase, ceruloplasmin) and the electron carriers (plastocyanin, stellacyanin, umecyanin, etc.). 

The ability to exist in more than one oxidation state allows transition-metal complexes to serve as the active site of enzymes whose function is to transfer electrons (39). A great deal of effort has been directed at understanding the mechanisms of electron transfer in metalloproteins, such as cytochromes and blue copper proteins (40). Of particular interest is the mechanism by which an electron can tunnel from a metal center that is imbedded in a protein matrix to a site on the outer surface of the protein (7). A discussion of current theories is given in this volume. 

Figure 8. Proposed electron transfer pathway in blue copper proteins. The plastocyanin wave function contours have been superimposed on the blue copper (type 1) site in ascorbate oxidase (40). The contour shows the substantial electron delocalization onto the cysteine Spir orbital that activates electron transfer to the trinuclear copper cluster at 12.5 A from the blue copper site. This low-energy, intense Cys Sp - Cu charge-transfer transition provides an effective hole superexchange mechanism for rapid long-range electron transfer between these sites (2, 3, 28).

Blue copper proteins are involved in electron transfer (ET) reactions in organisms ranging from bacteria to humans. In order to understand the contribution of the electronic structure to the ET function of these sites, it is useful to examine the three primary terms that contribute to the rate of ET, as described by the semi-classical Marcus equation (1) see also Long-range Electron Transfer in Biology). 

Figure 4 Cd PAC data—example, (a) Experimentally determined perturbation function that contains the information on the local structure and dynamics at the PAC probe site (data points with error bars and fit (fiiU line)).(b) Fourier transform of the experimental data (red) and of the fit (blue). This dataset was recorded for the cadnumn-substituted blue copper protein azurin. (After Figure 6 in )...

The type I copper sites function as electron transfer centers in the blue copper proteins and in multicopper enzymes, particularly oxidases (33). They are characterized by their intense blue color, their unusually small A values, and their very positive redox potentials (Table II). X-ray crystal structures of several blue copper proteins have been determined, notably plastocyanin (34), azurin (35), cucumber basic blue protein (36), and pseudoazurin (37). The active site structures show marked similarities but also distinct differences (Fig. 8). 

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