Dinuclear site Electron transfer

Cytochrome c oxidase is an enzyme that couples the one-electron oxidation of cytochrome c to the four-electron reduction of 02 and is thus a crucial component of respiration. Cytochrome c contains the redox-active heme c, while cytochrome c oxidase contains a dinuclear Cua redox site in subunit II and three redox-active sites in subunit I heme a, heme a3, and Cur. It is believed that heme a is an electron-transfer site, while heme a3 and Cur function together at the 02 reduction site. 

The high lability of bound N2 in [FeII(CN)5N2]3 regenerates the active site, namely the [FeII(CN)5H20]3 ion, which is able to further bind and process hydrazine. A more detailed kinetic study could be warranted for this interesting set of reactions. Some uncertainties still remain as to the nature of the intramolecular electron-transfer rate processes (91). At the employed concentration levels of the complex, the participation of mixtures of mononuclear and dinuclear complexes complicate the spectral evolution. Even the nature of the dinuclear intermediates (cyano- or hydrazino-bridged) could be put into question (probably both are involved, due to the labile interconversion equilibria). The participation of Fe(III) species, either in the mononuclear or dinuclear species, as reactive intermediate precursors of the formation of diazene and N2... 

The chemistry of cluster complexes, e.g. of the sort [FeitSi, (SR) i,] 2, is of particular interest since such complexes are known to be close representations or synthetic analogues of the redox centres present in various iron-sulphur proteins. It is important to know whether the valence electrons are localized or delocalized in such complexes - in fact several studies by e.s.r., n.m.r., and, more recently, resonance Raman spectroscopy have shown that such clusters are delocalized rather than trapped-valence species. This result is linked with the most important biophysical property of iron-sulphur proteins, viz. that of electron transfer. Rapid electron transfer is possible if any consequential geometric rearrangements around the metal atom sites are small, as implied by many resonance Raman results on such cluster complexes (cf. the small-displacement approximation, which provides a basis for enhancement to fundamental but not to overtone bands) (22). Initial studies of [MSi,]2- ions (M = Mo or W) (23,24) have since been supplemented by studies of dinuclear species e.g. [(PhS)2FeS2MS2]2 (25) and cluster species... 

This type of active site is also known as a mixed-valence copper site. Similarly to the type 3 site, it contains a dinuclear copper core, but both copper ions have a formal oxidation state of +1.5 in the oxidized form. This site exhibits a characteristic seven-line pattern in the EPR spectra and is purple colored. Both copper ions have a tetrahedral geometry and are bridged by two sulfur atoms of two cysteinyl residues. Each copper ion is also coordinated by a nitrogen atom from a histidine residue. The function of this site is long-range electron transfer, and it can be found, for example, in cytochrome c oxidase [12-14], and nitrous oxide reductase (Figure 5.1 e). 

Copper Hemocyanrn/Tyrosinase Models Copper Proteins with Dinuclear Active Sites Copper Proteins with Type 1 Sites Copper Proteins with Type 2 Sites Cytochrome Oxidase Electron Transfer Reactions Theory Long-range Electron Transfer in Biology Metal Ion Toxicity Metal-related Diseases of Genetic Origin Metallochaperones Metal Ion Homeostasis Nutritional Aspects of Metals Trace Elements. 

This is a remarkable reaction because the transition metal chemistry of N2O is sparse, especially with copper. Most N2O reductases are soluble, periplasmic homodimers however, there are examples of membrane-associated enzymes. " The best characterized N2O reductases are from Paracoccus denitrificans, Pseudomonas nautica, and Pseudomonas stutzeri, and most of the information presented here is derived from experiments on these enzymes. Where comparable data are available, N2O reductases from various organisms appear to be fairly similar, with the exception of the enzyme from Wolinella succinogenes, as noted above. The crystal stractmes of N2O reductase from P. nautica and more recently from P. denitrificans show two distinct copper clusters per subunit a bis-thiolate bridged dinuclear electron-transfer site (Cua), which is analogous to the Cua site in cytochrome c oxidase see Cyanide Complexes of the Transition Metals), and a novel four-copper cluster ligated by seven histidines, the catalytic copper site (Cuz), where N2O is thought to bind and be reduced. Cuz was proposed to be a copper-histidine cluster on the basis of the presence of nine strictly conserved histidine residues, and this was supported by a H NMR study that identified two non-CuA associated resonances that were assigned as copper-histidine N-H protons. ... 

Ascorbate oxidase is a tetramer each subunit has 552 amino acids and contains 4 copper ions, the type-I blue copper center and the adjacent trinuclear center (arranged as a type-n center and a type-in dinuclear center) separated by /S-sheets (Figure 20) °. Ascorbate is oxidized to dehydroascorbate by dioxygen however, it is not bound directly to the metal center to be oxidized, but is proposed to bind near the type-I Cu site which may facihtate electron transfer to oxygen, presumably in the tri-Cu cluster site. Since humans cannot synthesize ascorbic acid, conservation of this important compound is highly regulated. For example, the oxidized ascorbate can be transported into red blood... 

Modification of larger proteins with ruthenium complexes, while possible, have proven difficult. Fortunately, a ruthenium labeled partner such as Cc can be used to rapidly inject or remove an electron from the large protein complex, and thus study internal electron-transfer reactions. In a complementary approach, Nilsson found that the excited state of Ru(bpy)3 + can inject an electron into CcO. The ruthenium complex binds electrostatically to the protein in a location similar to that occupied by Cc. The initial site of electron transfer is the Cua site, as it is when Cc is the electron donor. The simplicity of this technique makes it very attractive since it eliminates any modification of the protein which might alter the structure. Sadoski etal. showed that significant improvements in the yield of electron transfer could be obtained with ruthenium complexes of higher charge. One specific complex used was the dinuclear complex [(bpy)2Ru(qpy)Ru(bpy)2] + (Figure 10). ... 

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