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Photo-catalytic oxidation of a di-nuclear manganese centre in an engineered bacterioferritin 'reaction centre'

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Date

2009

Authors

Conlan, Brendon
Cox, Nicholas
Su, Ji-Hu
Hillier, Warwick
Messinger, Johannes
Lubitz, Wolfgang
Dutton, Peter Leslie
Wydrzynski, Thomas

Journal Title

Journal ISSN

Volume Title

Publisher

Elsevier

Abstract

Photosynthesis involves the conversion of light into chemical energy through a series of electron transfer reactions within membrane-bound pigment/protein complexes. The Photosystem II (PSII) complex in plants, algae and cyanobacteria catalyse the oxidation of water to molecular O2. The complexity of PSII has thus far limited attempts to chemically replicate its function. Here we introduce a reverse engineering approach to build a simple, light-driven photo-catalyst based on the organization and function of the donor side of the PSII reaction centre. We have used bacterioferritin (BFR) (cytochrome b1) from Escherichia coli as the protein scaffold since it has several, inherently useful design features for engineering light-driven electron transport. Among these are: (i.) a di-iron binding site; (ii.) a potentially redox-active tyrosine residue; and (iii.) the ability to dimerise and form an inter-protein heme binding pocket within electron tunnelling distance of the di-iron binding site. Upon replacing the heme with the photoactive zinc-chlorin e6 (ZnCe6) molecule and the di-iron binding site with two manganese ions, we show that the two Mn ions bind as a weakly coupled di-nuclear Mn2II,II centre, and that ZnCe6 binds in stoichiometric amounts of 1:2 with respect to the dimeric form of BFR. Upon illumination the bound ZnCe6 initiates electron transfer, followed by oxidation of the di-nuclear Mn centre possibly via one of the inherent tyrosine residues in the vicinity of the Mn cluster. The light dependent loss of the MnII EPR signals and the formation of low field parallel mode Mn EPR signals are attributed to the formation of MnIII species. The formation of the MnIII is concomitant with consumption of oxygen. Our model is the first artificial reaction centre developed for the photo-catalytic oxidation of a di-metal site within a protein matrix which potentially mimics water oxidation centre (WOC) photo-assembly.

Description

Keywords

Keywords: bacterioferritin; chlorine; ferritin; hemoprotein; iron; manganese; scaffold protein; unclassified drug; zinc; article; binding site; bioengineering; catalysis; controlled study; electron spin resonance; electron transport; Escherichia coli; human; human Artificial photosynthesis; Bacterioferritin; Electron transfer; EPR; Manganese; Protein engineering; Zinc chlorin e6

Citation

URI

http://hdl.handle.net/1885/61632

Collections

ANU Research Publications

Source

Biochimica et Biophysica Acta: Bioenergetics

Type

Journal article

Book Title

Entity type

Access Statement

License Rights

DOI

10.1016/j.bbabio.2009.04.011

Restricted until

2037-12-31

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