Activation of the Cytochrome cd1 Nitrite Reductase from Paracoccus pantotrophus

Wonderen, Jessica H. van; Knight, Christopher T. G.; Oganesyan, Vasily S.; George, Simon J.; Zumft, Walter G.; Cheesman, Myles R.

doi:10.1074/jbc.m701242200

Cited by 15 publications

(11 citation statements)

References 58 publications

(87 reference statements)

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“…The correlation shows that i) when the g max signal increases, the average methyl chemical shift <δ> increases and ii) when the ligand field anisotropy V/Δ increases (from more axial to rhombic), the average methyl chemical shift <δ> decreases. The linear correlation holds fairly well when other experimental data ( g max , V/Δ and <δ>) available for similar cytochrome c proteins with His/Met axial ligation are included ( g max f (<δ>) with R = 0.93, V/Δ f (<δ>) with R = 0.95) such as horse cytochrome c 61, P. stutzeri c -551,47,65 P. ZoBell c -551,47,66 Rhodopseudomonas palustris c -2,67 and Saccharomyces cerevisiae iso-1 cyt c 47,68. However, the linear trend observed does not accommodate Bacillus pasteurii c -55369 and Rhodospirillum rubrum c -268, for which g max , V/Δ and <δ> values fall well outside the linear region.…”

Section: Resultssupporting

confidence: 57%

Modulation of the Ligand-Field Anisotropy in a Series of Ferric Low-Spin Cytochrome c Mutants derived from Pseudomonas aeruginosa Cytochrome c-551 and Nitrosomonas europaea Cytochrome c-552: A Nuclear Magnetic Resonance and Electron Paramagnetic Resonance Study

et al. 2008

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C-type cytochromes with histidine-methionine (His-Met) heme axial ligation play important roles in electron-transfer reactions and in enzymes. In this work two series of cytochrome c mutants derived from Pseudomonas aeruginosa (Pa c-551) and from the ammonia oxidizing bacterium Nitrosomonas europaea (Ne c-552) were engineered and over-expressed. In these proteins, point mutations were induced in a key residue (Asn64) near the Met axial ligand that have a considerable impact on both heme ligand-field strength and on the Met orientation and dynamics (fluxionality), as judged by lowtemperature electron paramagnetic resonance (EPR) and nuclear magnetic resonance (NMR) spectra. The Ne c-552 has a ferric low spin (S=1/2) EPR signal characterized by large g anisotropy with g max resonance at 3.34; a similar large g max value EPR signal is found in the mitochondrial Complex III cytochrome c 1 . In Ne c-552, deletion of Asn64 (NeN64Δ) changes the heme ligand-field from more axial to rhombic (small g anisotropy and g max at 3.13) and furthermore hinders the Met fluxionality present in the wild-type enzyme. In Pa c-551 (g max at 3.20) replacement of Asn64 with valine (PaN64V) induces a decrease in the axial strain (g max at 3.05) and changes the Met configuration. Another set of mutants prepared by insertion (ins) and/or deletion (Δ) of a valine residue adjacent to Asn64, resulting in modifications in the length of the axial Met-donating loop (NeV65Δ, NeG50N/V65Δ, PaN50G/V65ins), did not result in appreciable alterations of the originally weak (Ne c-552) or very weak axial (Pa c-551) field, but had an impact on Met orientation, fluxionality and relaxation dynamics. Comparison of the electronic fingerprints in the over-expressed proteins and their mutants reveals a linear relation between axial strain and average paramagnetic heme methyl shifts, irrespective of Met orientation or dynamics. Thus, for these His-Met axially coordinated Fe(III) the large g max value EPR signal does not represent a special case as is observed for bis-His axially coordinated Fe(III) with the two His planes perpendicular to each other.

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Section: Resultssupporting

confidence: 57%

Modulation of the Ligand-Field Anisotropy in a Series of Ferric Low-Spin Cytochrome c Mutants derived from Pseudomonas aeruginosa Cytochrome c-551 and Nitrosomonas europaea Cytochrome c-552: A Nuclear Magnetic Resonance and Electron Paramagnetic Resonance Study

et al. 2008

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“…No peak between 550 and 630 nm was seen for the Y25S enzyme with either nitrite or NO bound, further indicating that the 620 nm peak does not arise from either of these ligands bound to ferric d 1 heme. Recent work has invoked the possibility of electron donation from an amino acid side chain during nitrite reduction by cytochrome cd 1 (20), and therefore formation of cFe(II)⅐d 1 Fe(II)-NO was also addressed. However, when the 130-s sample was subjected to EPR, no signal arising from Fe(II)-NO was observed.…”

Section: Discussionmentioning

confidence: 99%

Very Early Reaction Intermediates Detected by Microsecond Time Scale Kinetics of Cytochrome cd1-catalyzed Reduction of Nitrite

Sam

Strampraad

Vries

et al. 2008

Journal of Biological Chemistry

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Paracoccus pantotrophus cytochrome cd 1 is a nitrite reductase found in the periplasm of many denitrifying bacteria. It catalyzes the reduction of nitrite to nitric oxide during the denitrification part of the biological nitrogen cycle. Previous studies of early millisecond intermediates in the nitrite reduction reaction have shown, by comparison with pH 7.0, that at the optimum pH, approximately pH 6, the earliest intermediates were lost in the dead time of the instrument. Access to early time points (ϳ100 s) through use of an ultra-rapid mixing device has identified a spectroscopically novel intermediate, assigned as the Michaelis complex, formed from reaction of fully reduced enzyme with nitrite. Spectroscopic observation of the subsequent transformation of this species has provided data that demand reappraisal of the general belief that the two subunits of the enzyme function independently.

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“…19 The disproportionation of NO 2 -readily occurs in strongly acidic solution, but the rate is extremely low at pH g7. 20 Although the reaction is not promoted by heme proteins, 3 it was observed in a few model ferrihemes with exclusion of water.…”

mentioning

confidence: 99%

Formation of Nitric Oxide from Nitrite by the Ferriheme b Protein Nitrophorin 7

Knipp

2009

J. Am. Chem. Soc.

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Recently, the conversion of nitrite into NO by certain heme proteins, in particular hemoglobin, gained much interest as a physiologically important source of NO in human tissue. However, in an aqueous environment, nitrite reduction at an iron porphyrin occurs either through oxidation of ferroheme to ferriheme or with the assistance of a second substrate molecule. Here we report on the reduction of nitrite in the absence of a second substrate at the heme center of the ferriheme protein nitrophorin 7 (NP7) resulting in the formation of NO and restoration of the ferriheme center. The product was spectroscopically characterized, in particular by resonance Raman and FT-IR spectroscopy. Performing the reaction in the presence of the NO trap 2-(4-trimethylammonio)phenyl-4,4,5,5-tetramethylimidazoline-1-oxyl 3-oxide (TMA-PTIO) revealed that continuous NO production is possible, i.e., that NP7 is fully restored upon a single turnover. Thus, NP7 is the first case of a b-type heme that performs reduction of nitrite as a single substrate out of the iron(III) state.

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Activation of the Cytochrome cd1 Nitrite Reductase from Paracoccus pantotrophus

Cited by 15 publications

References 58 publications

Modulation of the Ligand-Field Anisotropy in a Series of Ferric Low-Spin Cytochrome c Mutants derived from Pseudomonas aeruginosa Cytochrome c-551 and Nitrosomonas europaea Cytochrome c-552: A Nuclear Magnetic Resonance and Electron Paramagnetic Resonance Study

Modulation of the Ligand-Field Anisotropy in a Series of Ferric Low-Spin Cytochrome c Mutants derived from Pseudomonas aeruginosa Cytochrome c-551 and Nitrosomonas europaea Cytochrome c-552: A Nuclear Magnetic Resonance and Electron Paramagnetic Resonance Study

Very Early Reaction Intermediates Detected by Microsecond Time Scale Kinetics of Cytochrome cd1-catalyzed Reduction of Nitrite

Formation of Nitric Oxide from Nitrite by the Ferriheme b Protein Nitrophorin 7

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