36 research outputs found

    Site of action of a halogenated 4-hydroxypyridine on ferredoxin-catalysed cyclic photophosphorylation

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    AbstractTetrabromo-4-hydroxypyridine (J820) inhibited ferredoxin-catalysed cyclic photophosphorylation at micromolar concentrations but did not inhibit or uncouple the AQS-catalysed system. At 2 μM it did not abolish the slow phase of the electrochromic shift or affect the turnover of cytochromes b-563 and f. At higher concentrations (10 μM) it decreased the rate of re-reduction of cytochrome f, whilst inhibiting the reduction of cytochrome b-563. It is concluded that tetrabromo-4-hydroxpyridine does not bind to the quinone reduction site of the cytochrome bf complex, but inhibits the putative ferredoxin-plastoquinone reductase

    The role of a disulfide bridge in the stability and folding kinetics of Arabidopsis thaliana cytochrome c6A

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    Cytochrome c 6A is a eukaryotic member of the Class I cytochrome c family possessing a high structural homology with photosynthetic cytochrome c 6 from cyanobacteria, but structurally and functionally distinct through the presence of a disulfide bond and a heme mid-point redox potential of + 71 mV (vs normal hydrogen electrode). The disulfide bond is part of a loop insertion peptide that forms a cap-like structure on top of the core α-helical fold. We have investigated the contribution of the disulfide bond to thermodynamic stability and (un)folding kinetics in cytochrome c 6A from Arabidopsis thaliana by making comparison with a photosynthetic cytochrome c 6 from Phormidium laminosum and through a mutant in which the Cys residues have been replaced with Ser residues (C67/73S). We find that the disulfide bond makes a significant contribution to overall stability in both the ferric and ferrous heme states. Both cytochromes c 6A and c 6 fold rapidly at neutral pH through an on-pathway intermediate. The unfolding rate for the C67/73S variant is significantly increased indicating that the formation of this region occurs late in the folding pathway. We conclude that the disulfide bridge in cytochrome c 6A acts as a conformational restraint in both the folding intermediate and native state of the protein and that it likely serves a structural rather than a previously proposed catalytic role. © 2011 Elsevier B.V. All rights reserved

    Development of Photosynthetic Electron Transport in Greening Barley

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    Oxygen Evolution in Photosynthesis

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    Complex of Plastocyanin and Cytochrome c

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    Redox titration of the slow ΔA518 in chloroplasts

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    Structural and kinetic studies of imidazole binding to two members of the cytochrome c 6 family reveal an important role for a conserved heme pocket residue

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    The amino acid at position 51 in the cytochrome c 6 family is responsible for modulating over 100 mV of heme midpoint redox potential. As part of the present work, the X-ray structure of the imidazole adduct of the photosynthetic cytochrome c 6 Q51V variant from Phormidium laminosum has been determined. The structure reveals the axial Met ligand is dissociated from the heme iron but remains inside the heme pocket and the Ω-loop housing the Met ligand is stabilized through polar interactions with the imidazole and heme propionate-6. The latter is possible owing to a 180° rotation of both heme propionates upon imidazole binding. From equilibrium and kinetic studies, a Val residue at position 51 increases the stability of the Fe-S(Met) interaction and also affects the dynamics associated with imidazole binding. In this respect, the k obs for imidazole binding to Arabidopsis thaliana cytochrome c 6A, which has a Val at the position equivalent to position 51 in photosynthetic cytochrome c 6, was found to be independent of imidazole concentration, indicating that the binding process is limited by the Met dissociation rate constant (about 1 s -1). For the cytochrome c 6 Q51V variant, imidazole binding was suppressed in comparison with the wild-type protein and the V52Q variant of cytochrome c 6A was found to bind imidazole readily. We conclude that the residue type at position 51/52 in the cytochrome c 6 family is additionally responsible for tuning the stability of the heme iron-Met bond and the dynamic properties of the ferric protein fold associated with endogenous ligand binding. © 2011 SBIC
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