The Semiquinone at the Qi Site of the bc1 Complex Explored Using HYSCORE Spectroscopy and Specific Isotopic Labeling of Ubiquinone in Rhodobacter sphaeroides via 13C Methionine and Construction of a Methionine Auxotroph

Hong, Sung Il; Almeida, Wagner B. De; Taguchi, Alexander T.; Samoilova, Rimma I.; Gennis, Robert B.; O’Malley, Patrick J.; Dikanov, Sergei A.; Crofts, Antony R.

doi:10.1021/bi500654y

Cited by 13 publications

(12 citation statements)

References 52 publications

(159 reference statements)

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“…While this scenario is possible, the other option is that the proton transfers are tightly coupled to separate e − transfers ( Fig. 1B ) as recently suggested by quantum mechanics calculations 16 . Accordingly, the half-protonated SQ ( Fig.…”

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confidence: 86%

“…To address this issue, the bacterial cyt bc 1 complex was studied afresh using explicitly set up MD simulations ( Table 1 ). Because only the anionic SQ has been detected using frozen electron paramagnetic resonance experiments at the Q i -site 12 13 14 15 16 , the substrate has been presumed to acquire both of the electrons (dianionic state) before accepting the two protons concomitantly 17 . While this scenario is possible, the other option is that the proton transfers are tightly coupled to separate e − transfers ( Fig.…”

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confidence: 99%

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Atomistic determinants of co-enzyme Q reduction at the Qi-site of the cytochrome bc1 complex

Postila

Kaszuba

Kuleta

et al. 2016

Sci Rep

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The cytochrome (cyt) bc1 complex is an integral component of the respiratory electron transfer chain sustaining the energy needs of organisms ranging from humans to bacteria. Due to its ubiquitous role in the energy metabolism, both the oxidation and reduction of the enzyme’s substrate co-enzyme Q has been studied vigorously. Here, this vast amount of data is reassessed after probing the substrate reduction steps at the Qi-site of the cyt bc1 complex of Rhodobacter capsulatus using atomistic molecular dynamics simulations. The simulations suggest that the Lys251 side chain could rotate into the Qi-site to facilitate binding of half-protonated semiquinone – a reaction intermediate that is potentially formed during substrate reduction. At this bent pose, the Lys251 forms a salt bridge with the Asp252, thus making direct proton transfer possible. In the neutral state, the lysine side chain stays close to the conserved binding location of cardiolipin (CL). This back-and-forth motion between the CL and Asp252 indicates that Lys251 functions as a proton shuttle controlled by pH-dependent negative feedback. The CL/K/D switching, which represents a refinement to the previously described CL/K pathway, fine-tunes the proton transfer process. Lastly, the simulation data was used to formulate a mechanism for reducing the substrate at the Qi-site.

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confidence: 86%

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confidence: 99%

Atomistic determinants of co-enzyme Q reduction at the Qi-site of the cytochrome bc1 complex

Postila

Kaszuba

Kuleta

et al. 2016

Sci Rep

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“…A stable intermediate semiquinone at the Qn site has been studied, see for example, ref. and references therein. As semiquinones have been implicated in ROS production, these discussions are not purely academic.…”

Section: Looking At Complex III In the Light Of Ros Formationmentioning

confidence: 99%

Can All Major ROS Forming Sites of the Respiratory Chain Be Activated By High FADH₂/NADH Ratios?

Speijer

2018

BioEssays

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Aspects of peroxisome evolution, uncoupling, carnitine shuttles, supercomplex formation, and missing neuronal fatty acid oxidation (FAO) are linked to reactive oxygen species (ROS) formation in respiratory chains. Oxidation of substrates with high FADH 2 /NADH (F/N) ratios (e.g., FAs) initiate ROS formation in Complex I due to insufficient availability of its electron acceptor (Q) and reverse electron transport from QH 2 , e.g., during FAO or glycerol-3-phosphate shuttle use. Here it is proposed that the Q-cycle of Complex III contributes to enhanced ROS formation going from low F/N ratio substrates (glucose) to high F/N substrates. This contribution is twofold: 1) Complex III uses Q as substrate, thus also competing with Complex I; 2) Complex III itself will produce more ROS under these conditions. I link this scenario to the universally observed Complex III dimerization. The Q-cycle of Complex III thus again illustrates the tension between efficient ATP generation and endogenous ROS formation. This model can explain recent findings concerning succinate and ROS-induced uncoupling.

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“…[42] In addition, as imilar approach using selectively 13 Clabeled methionines allowed selective 13 Ce nrichmento ft he methyl and methoxy substituents of ubisemiquinoneb ound at the cyt bo 3 Q H site from E. coli or at the bc 1 complex Q i site from Rhodobacter sphaeroides. [52,53] NarGHI-enriched inner membrane vesicles were purified from the methionine-deficient strain mentioned above, titrated, and studied by EPR spectroscopy.T he cw EPR spectrumo fasample poiseda t À158 mV is shown in Figure 3. It shows an intense unstructured isotropic radical signal centered at g av % 2.0045w ith a peak-to-peak line width of about 0.6 mT assigned to NarGHIbound MSK D with a 2 H-labeled methyl group, hereafter referred to as C 2 H 3 -MSK D .T he EPR peak-to-peak line width of C 2 H 3 -MSK D decreases by % 0.2 mT with respect to that measured for unlabeled MSK D (Figure 3, dashed trace),i ndicating as ignificant contribution of the methyl protons hyperfine coupling to the MSK D EPR linewidth.…”

Section: Hh Yscore Spectroscopy On Narghi-bound Msk From Methioninementioning

confidence: 99%

“…[42] In addition, as imilar approach using selectively 13 Clabeled methionines allowed selective 13 Ce nrichmento ft he methyl and methoxy substituents of ubisemiquinoneb ound at the cyt bo 3 Q H site from E. coli or at the bc 1 complex Q i site from Rhodobacter sphaeroides. [52,53] NarGHI-enriched inner membrane vesicles were purified from the methionine-deficient strain mentioned above, titrated, and studied by EPR spectroscopy.T he cw EPR spectrumo fasample poiseda t Figure 2. Contour presentationsoft he low-frequency part of representative HYSCORE spectrao fMSK D by using eitheru nenriched NarGHI (A),u niform 15 Ne nrichment of NarGHI (B), selectively 15 N-labeled NarGHI on His Nd (C), or selectively 15 N-labeled NarGHI on LysNz (D).…”

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confidence: 99%

Probing the Menasemiquinone Binding Mode to Nitrate Reductase A by Selective ²H and ¹⁵N Labeling, HYSCORE Spectroscopy, and DFT Modeling

et al. 2017

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In vivo specific isotope labeling at the residue or substituent level is used to probe menasemiquinone (MSK) binding to the quinol oxidation site of respiratory nitrate reductase A (NarGHI) from E. coli. 15N selective labeling of His15Nδ or Lys15Nζ in combination with hyperfine sublevel correlation (HYSCORE) spectroscopy unambiguously identified His15Nδ as the direct hydrogen‐bond donor to the radical. In contrast, an essentially anisotropic coupling to Lys15Nζ consistent with a through‐space magnetic interaction was resolved. This suggests that MSK does not form a hydrogen bond with the side chain of the nearby Lys86 residue. In addition, selective 2H labeling of the menaquinone methyl ring substituent allows unambiguous characterization of the 2H—and hence of the 1H—methyl isotropic hyperfine coupling by 2H HYSCORE. DFT calculations show that a simple molecular model consisting of an imidazole Nδ atom in a hydrogen‐bond interaction with a MSK radical anion satisfactorily accounts for the available spectroscopic data. These results support our previously proposed one‐sided binding model for MSK to NarGHI through a single short hydrogen bond to the Nδ of His66, one of the distal heme axial ligands. This work establishes the basis for future investigations aimed at determining the functional relevance of this peculiar binding mode.

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The Semiquinone at the Q_i Site of the bc₁ Complex Explored Using HYSCORE Spectroscopy and Specific Isotopic Labeling of Ubiquinone in Rhodobacter sphaeroides via ¹³C Methionine and Construction of a Methionine Auxotroph

Cited by 13 publications

References 52 publications

Atomistic determinants of co-enzyme Q reduction at the Qi-site of the cytochrome bc1 complex

Atomistic determinants of co-enzyme Q reduction at the Qi-site of the cytochrome bc1 complex

Can All Major ROS Forming Sites of the Respiratory Chain Be Activated By High FADH₂/NADH Ratios?

Probing the Menasemiquinone Binding Mode to Nitrate Reductase A by Selective ²H and ¹⁵N Labeling, HYSCORE Spectroscopy, and DFT Modeling

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The Semiquinone at the Qi Site of the bc1 Complex Explored Using HYSCORE Spectroscopy and Specific Isotopic Labeling of Ubiquinone in Rhodobacter sphaeroides via 13C Methionine and Construction of a Methionine Auxotroph

Cited by 13 publications

References 52 publications

Atomistic determinants of co-enzyme Q reduction at the Qi-site of the cytochrome bc1 complex

Atomistic determinants of co-enzyme Q reduction at the Qi-site of the cytochrome bc1 complex

Can All Major ROS Forming Sites of the Respiratory Chain Be Activated By High FADH2/NADH Ratios?

Probing the Menasemiquinone Binding Mode to Nitrate Reductase A by Selective 2H and 15N Labeling, HYSCORE Spectroscopy, and DFT Modeling

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The Semiquinone at the Q_i Site of the bc₁ Complex Explored Using HYSCORE Spectroscopy and Specific Isotopic Labeling of Ubiquinone in Rhodobacter sphaeroides via ¹³C Methionine and Construction of a Methionine Auxotroph

Can All Major ROS Forming Sites of the Respiratory Chain Be Activated By High FADH₂/NADH Ratios?

Probing the Menasemiquinone Binding Mode to Nitrate Reductase A by Selective ²H and ¹⁵N Labeling, HYSCORE Spectroscopy, and DFT Modeling