Single-molecule study of redox control involved in establishing the spinach plastocyanin-cytochrome b6f electron transfer complex

Single-molecule study of redox control involved in establishing the spinach plastocyanin-cytochrome b6f electron transfer complex

Small diffusible redox proteins play a ubiquitous role in bioenergetic systems, facilitating electron transfer (ET) between membrane bound complexes. Sustaining high ET turnover rates requires that the association between extrinsic and membrane-bound partners is highly specific, yet also sufficientl...

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Published in:Biochimica et biophysica acta. Bioenergetics Vol. 1860; no. 7; pp. 591 - 599
Main Authors: Mayneord, Guy E., Vasilev, Cvetelin, Malone, Lorna A., Swainsbury, David J.K., Hunter, C. Neil, Johnson, Matthew P.
Format: Journal Article
Language:English
Published: Elsevier B.V 01-07-2019
Subjects:
Atomic force microscopy
Electron transfer, cytochrome b6f
Photosynthesis
Plastocyanin
Atomic force microscopy
Plastocyanin
Electron transfer, cytochrome b6f
Photosynthesis
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Summary:Small diffusible redox proteins play a ubiquitous role in bioenergetic systems, facilitating electron transfer (ET) between membrane bound complexes. Sustaining high ET turnover rates requires that the association between extrinsic and membrane-bound partners is highly specific, yet also sufficiently weak to promote rapid post-ET separation. In oxygenic photosynthesis the small soluble electron carrier protein plastocyanin (Pc) shuttles electrons between the membrane integral cytochrome b6f (cytb6f) and photosystem I (PSI) complexes. Here we use peak-force quantitative nanomechanical mapping (PF-QNM) atomic force microscopy (AFM) to quantify the dynamic forces involved in transient interactions between cognate ET partners. An AFM probe functionalised with Pc molecules is brought into contact with cytb6f complexes, immobilised on a planar silicon surface. PF-QNM interrogates the unbinding force of the cytb6f-Pc interactions at the single molecule level with picoNewton force resolution and on a time scale comparable to the ET time in vivo (ca. 120 μs). Using this approach, we show that although the unbinding force remains unchanged the interaction frequency increases over five-fold when Pc and cytb6f are in opposite redox states, so complementary charges on the cytb6f and Pc cofactors likely contribute to the electrostatic forces that initiate formation of the ET complex. These results suggest that formation of the docking interface is under redox state control, which lowers the probability of unproductive encounters between Pc and cytb6f molecules in the same redox state, ensuring the efficiency and directionality of this central reaction in the ‘Z-scheme’ of photosynthetic ET. [Display omitted] •Single molecule force spectroscopy was applied to study the cytochrome b6f – plastocyanin interaction.•Plastocyanin was attached to the AFM probe and cytochrome b6f to a silicon surface.•Their frequency of interaction was highest when they inhabited opposing redox states e.g. oxidised/reduced.•When in the same redox state (e.g. oxidised/oxidised) their interaction frequency was 5 fold lower.•Nature likely uses this phenomenon to avoid unproductive encounters between molecules in the same redox state.
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ISSN:0005-2728
1879-2650
DOI:10.1016/j.bbabio.2019.06.013