Interprotein electron transfer from cytochrome<i>c</i><sub>2</sub>to photosynthetic reaction center: Tunneling across an aqueous interface

Miyashita, Osamu; Okamura, M. Y.; Onuchic, José N.

doi:10.1073/pnas.0409600102

Cited by 98 publications

(101 citation statements)

References 54 publications

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“…Notably, a similar water channel containing five ordered water molecules reaching from the protein surface to the heme was revealed in cytochrome f and showed to be crucial for its in vivo electron transfer function (40,41). In some models, it was demonstrated that ordered water molecules can directly facilitate electron transfer, working as an "electron wire" (42,43). Therefore, the highly ordered water molecules in KillerRed could possibly play a role of electron wire, conducting electrons from the attacked external molecule.…”

Section: Discussionmentioning

confidence: 99%

Structural Basis for Phototoxicity of the Genetically Encoded Photosensitizer KillerRed

Pletnev

Gurskaya

Pletneva

et al. 2009

Journal of Biological Chemistry

128

168

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KillerRed is the only known fluorescent protein that demonstrates notable phototoxicity, exceeding that of the other green and red fluorescent proteins by at least 1,000-fold. KillerRed could serve as an instrument to inactivate target proteins or to kill cell populations in photodynamic therapy. However, the nature of KillerRed phototoxicity has remained unclear, impeding the development of more phototoxic variants. Here we present the results of a high resolution crystallographic study of KillerRed in the active fluorescent and in the photobleached non-fluorescent states. A unique and striking feature of the structure is a waterfilled channel reaching the chromophore area from the end cap of the ␤-barrel that is probably one of the key structural features responsible for phototoxicity. A study of the structure-function relationship of KillerRed, supported by structure-based, site-directed mutagenesis, has also revealed the key residues most likely responsible for the phototoxic effect. In particular, Glu 68 and Ser 119, located adjacent to the chromophore, have been assigned as the primary trigger of the reaction chain. The green fluorescent protein (GFP)2 and related proteins have become efficient noninvasive tools in cell biology and biomedicine for visualizing and monitoring the internal processes within cells or whole organisms (1-8). The multicolor labeling technologies, based on fluorescent proteins (FPs), have found important biomedical applications in the studies of various aspects of cancer, including primary tumor growth, tumor cell motility and invasion, metastatic seeding, colonization, and angiogenesis (9 -11).The recent development of the first genetically encoded photosensitizer, KillerRed (SWISS-PROT/TrEMBL data base sequence ID Q2TCH5), a highly phototoxic red fluorescent protein (12, 13), opened a new area of FP application. KillerRed is a red fluorescent protein characterized by excitation and emission maxima at 585 and 610 nm, respectively. This genetic variant was engineered from non-fluorescent and non-phototoxic chromoprotein anm2CP from Hydrozoa jellyfish (sequence ID Q6RYS4). Upon irradiation by green light at the wavelength of 520 -590 nm, KillerRed generates the reactive oxygen species (ROS), accompanied by profound self photobleaching. The ROS-induced phototoxicity of KillerRed is at least 3 orders of magnitude higher than that of other fluorescent proteins exhibiting low background phototoxicity (12). Such a unique property of KillerRed could find use in light-induced inactivation of target proteins and in precise cell killing. Unlike chemical photosensitizers, KillerRed can be directly expressed by a target cell, both individually and in fusion with a target protein. The most exciting future application of KillerRed may be in photodynamic therapy of cancer. This phototoxic agent, precisely delivered to solid tumors by a viral vector, could serve as an intrinsically generated photosensitizer, causing light-induced tumor destruction. Therefore, understanding the relationship between...

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Section: Discussionmentioning

confidence: 99%

Structural Basis for Phototoxicity of the Genetically Encoded Photosensitizer KillerRed

Pletnev

Gurskaya

Pletneva

et al. 2009

Journal of Biological Chemistry

128

168

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“…However, the transfer rate of N3 → N1b (∼10 3 s −1 ) is slower than the highest estimate, and N5 → N6a (∼10 s −1 ) is drastically slower than the reported rates, which indicates that an important factor is missing in the model. The pathway analysis shows that the two slowest processes N5 → N6a and N3 → N1b are controlled by the rate of electron tunneling across protein subunit boundaries where internal water molecules should be present (14). In the reported structure, however, the intervening water is not seen, which suggests its significant mobility.…”

mentioning

confidence: 84%

“…11). However, in that study, the internal water has not been taken into account, whereas it is known that water in proteins is capable of accelerating electron transfer (12)(13)(14)(15). In this paper we use state-of-the-art electronic structure calculations to show that the mechanism of electron transfer is quantum mechanical tunneling, as in the rest of electron transport chain; the water between subunits of complex I plays the critical role in mediating electron transport.…”

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confidence: 99%

Electron tunneling in respiratory complex I

Hayashi

Stuchebrukhov

2010

Proc. Natl. Acad. Sci. U.S.A.

119

120

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NADH:ubiquinone oxidoreductase (complex I) plays a central role in the respiratory electron transport chain by coupling the transfer of electrons from NADH to ubiquinone to the creation of the proton gradient across the membrane necessary for ATP synthesis. Here the atomistic details of electronic wiring of all Fe/S clusters in complex I are revealed by using the tunneling current theory and computer simulations; both density functional theory and semiempirical electronic structure methods were used to examine antiferromagnetically coupled spin states and corresponding tunneling wave functions. Distinct electron tunneling pathways between neighboring Fe/S clusters are identified; the pathways primarily consist of two cysteine ligands and one additional key residue. Internal water between protein subunits is identified as an essential mediator enhancing the overall electron transfer rate by almost three orders of magnitude to achieve a physiologically significant value. The identified key residues are further characterized by sensitivity of electron transfer rates to their mutations, examined in simulations, and their conservation among complex I homologues. The unusual electronic structure properties of Fe 4 S 4 clusters in complex I explain their remarkable efficiency of electron transfer.electron transfer in proteins | respiratory chain | iron-sulfur clusters N ADH:ubiquinone oxidoreductase (complex I) is a large L-shaped membrane-bound enzyme involved in cellular respiration that catalyzes the oxidation of NADH and the reduction of ubiquinone in mitochondria and respiring bacteria (1-3). This reaction involves the transfer of electrons over approximately 90 Å from NADH bound to the hydrophilic domain to ubiquinone in or near the hydrophobic membrane-bound domain of complex I (4). In turn, the reaction provides the driving force for translocation of four protons across the membrane, thus generating, in part, the proton gradient necessary for ATP synthesis (5). Complex I defects are the cause of several neurodegenerative diseases including Parkinson disease, Alzheimer's disease, and Huntington disease (6).The transfer of electrons from NADH to ubiquinone is facilitated by flavin mononucleotide (FMN), two binuclear (2Fe-2S) iron-sulfur clusters (N1a and N1b), and six tetranuclear (4Fe-4S) iron-sulfur clusters (N3, N4, N5, N6a, N6b, and N2) (Fig. 1A). NADH, a two-electron donor, initially passes both electrons, as hydride, to the FMN cofactor. From FMN one electron enters a transport chain leading to the ubiquinone-binding site; the second electron enters a side path to N1a that appears to serve as a control mechanism to prevent generation of superoxide ions (4).The crystal structure of hydrophilic domain of complex I from Thermus thermophilus was reported in 2006 (4), and recently the whole architecture of the enzyme has been revealed (7); however, until now, the atomistic details of electron transfer along the chain of Fe/S metal clusters have remained unknown. Recently, a hopping (stepwise) electron transfer (...

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“…They are formed from a nucleus called a Heme. At the centre of the Heme is an iron atom which can pass from the second to the third oxidation level and this atom transfers an electron at each level change (Miyashita et al, 2005). Around this structure is an amino-acid chain which has no direct function.…”

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confidence: 99%

Quantum Physics in Living Matter: From Quantum Biology to Quantum Neurobiology

Tarlacı¹

2011

NeuroQuantology

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For years, quantum physics was seen as the physics of non-living matter. Thus, when biological living things were discussed, this sequence always came to the fore: biology →organism→ organs→ tissue→ biochemistry→ physics→ classical mechanics + quantum mechanics. It can be seen that there was a reduction to the lower structures and that at the base one reaches the level of particles such as atoms and molecules. But when the physico-chemical level is reached, it can be seen that many quantum mechanical events are taking place in living things, and that in fact these are quite normal reactions.

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Interprotein electron transfer from cytochromec₂to photosynthetic reaction center: Tunneling across an aqueous interface

Cited by 98 publications

References 54 publications

Structural Basis for Phototoxicity of the Genetically Encoded Photosensitizer KillerRed

Structural Basis for Phototoxicity of the Genetically Encoded Photosensitizer KillerRed

Electron tunneling in respiratory complex I

Quantum Physics in Living Matter: From Quantum Biology to Quantum Neurobiology

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Interprotein electron transfer from cytochromec2to photosynthetic reaction center: Tunneling across an aqueous interface

Cited by 98 publications

References 54 publications

Structural Basis for Phototoxicity of the Genetically Encoded Photosensitizer KillerRed

Structural Basis for Phototoxicity of the Genetically Encoded Photosensitizer KillerRed

Electron tunneling in respiratory complex I

Quantum Physics in Living Matter: From Quantum Biology to Quantum Neurobiology

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Product

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Interprotein electron transfer from cytochromec₂to photosynthetic reaction center: Tunneling across an aqueous interface