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1.
Feng C Wilson HL Hurley JK Hazzard JT Tollin G Rajagopalan KV Enemark JH 《The Journal of biological chemistry》2003,278(5):2913-2920
Tyrosine 343 in human sulfite oxidase (SO) is conserved in all SOs sequenced to date. Intramolecular electron transfer (IET) rates between reduced heme (Fe(II)) and oxidized molybdenum (Mo(VI)) in the recombinant wild-type and Y343F human SO were measured for the first time by flash photolysis. The IET rate in wild-type human SO at pH 7.4 is about 37% of that in chicken SO with a similar decrease in k(cat). Steady-state kinetic analysis of the Y343F mutant showed an increase in K(m)(sulfite) and a decrease in k(cat) resulting in a 23-fold attenuation in the specificity constant k(cat)/K(m)(sulfite) at the optimum pH value of 8.25. This indicates that Tyr-343 is involved in the binding of the substrate and catalysis within the molybdenum active site. Furthermore, the IET rate constant in the mutant at pH 6.0 is only about one-tenth that of the wild-type enzyme, suggesting that the OH group of Tyr-343 is vital for efficient IET in SO. The pH dependences of IET rate constants in the wild-type and mutant SO are consistent with the previously proposed coupled electron-proton transfer mechanism. 相似文献
2.
Feng C Wilson HL Tollin G Astashkin AV Hazzard JT Rajagopalan KV Enemark JH 《Biochemistry》2005,44(42):13734-13743
Mutations G473D and A208D were identified in patients with isolated sulfite oxidase (SO) deficiency, and the equivalent amino acids (G451 and A186, respectively) have been localized to the vicinity of the molybdopterin active site in the X-ray structure of chicken SO [Kisker, C., Schindelin, H., Pacheco, A., Wehbi, W., Garrett, R. M., Rajagopalan, K. V., Enemark, J. H., and Rees, D. C. (1997) Cell 91, 973-983]. To assess the effects of these mutations in human SO, steady-state kinetic studies of enzyme turnover and laser flash photolysis measurements of intramolecular electron transfer (IET) rate constants between the reduced heme [Fe(II)] and Mo(VI) centers were carried out in the recombinant G473D, G473A, G473W, G473D/R212A, and A208D human SO mutants. In the G473D and A208D mutants, the IET rate constants at pH 6.0 are decreased by 3 orders of magnitude relative to that of the wild type. Steady-state kinetic measurements indicate that the IET process is the rate-limiting step in the catalytic cycle of these two mutants. Thus, the large decreases in the IET rate constants and the kcat values, and the large increases in the Km(sulfite) values, rationalize the fatal impact of these mutations. Far-UV CD spectra of G473D indicate that the protein backbone conformation is remarkably changed, and the sedimentation equilibrium indicates that the protein is monomeric. Furthermore, EPR studies also suggest that the active site structure of the Mo(V) form of A208D is different from that of the wild type. In contrast, similar studies on G473A show that it is dimeric, that its Mo(V) active site structure is similar to that of the wild type, and that its IET rate constant is only 2.6-fold smaller than that of the wild type. IET in G473W is severely impaired, and no IET is observed for G473D/R212A. In chicken SO, the equivalent residues (G451 and A186) are both buried inside the protein. Thus, for human SO, the mutations to charged residues at the equivalent sites most likely cause crucial global or localized structural changes, and expose an alternative docking site that may compete with the Mo domain for docking of the heme, thereby retarding IET and efficient catalytic turnover of the sulfite oxidation reaction. 相似文献
3.
Johnson-Winters K Nordstrom AR Davis AC Tollin G Enemark JH 《Metallomics : integrated biometal science》2010,2(11):766-770
Sulfite oxidase (SO) is a molybdenum-cofactor-dependent enzyme that catalyzes the oxidation of sulfite to sulfate, the final step in the catabolism of the sulfur-containing amino acids, cysteine and methionine. The catalytic mechanism of vertebrate SO involves intramolecular electron transfer (IET) from molybdenum to the integral b-type heme of SO and then to exogenous cytochrome c. However, the crystal structure of chicken sulfite oxidase (CSO) has shown that there is a 32 ? distance between the Fe and Mo atoms of the respective heme and molybdenum domains, which are connected by a flexible polypeptide tether. This distance is too long to be consistent with the measured IET rates. Previous studies have shown that IET is viscosity dependent (Feng et al., Biochemistry, 2002, 41, 5816) and also dependent upon the flexibility and length of the tether (Johnson-Winters et al., Biochemistry, 2010, 49, 1290). Since IET in CSO is more rapid than in human sulfite oxidase (HSO) (Feng et al., Biochemistry, 2003, 42, 12235) the tether sequence of HSO has been mutated into that of CSO, and the resultant chimeric HSO enzyme investigated by laser flash photolysis and steady-state kinetics in order to study the specificity of the tether sequence of SO on the kinetic properties. Surprisingly, the IET kinetics of the chimeric HSO protein with the CSO tether sequence are slower than wildtype HSO. This observation raises the possibility that the composition of the non-conserved tether sequence of animal SOs may be optimized for individual species. 相似文献
4.
Essential role of conserved arginine 160 in intramolecular electron transfer in human sulfite oxidase 总被引:1,自引:0,他引:1
Feng C Wilson HL Hurley JK Hazzard JT Tollin G Rajagopalan KV Enemark JH 《Biochemistry》2003,42(42):12235-12242
Arginine 160 in human sulfite oxidase (SO) is conserved in all SO species sequenced to date. Previous steady-state kinetic studies of the R160Q human SO mutant showed a remarkable decrease in k(cat)/K(m)(sulfite) of nearly 1000-fold, which suggests that Arg 160 in human SO makes an important contribution to the binding of sulfite near the molybdenum cofactor [Garrett, R. M., Johnson, J. L., Graf, T. N., Feigenbaum, A., Rajagopalan, K. V. (1998) Proc. Natl. Acad. Sci. U.S.A. 95, 6394-6398]. In the crystal structure of chicken SO, Arg 138, the equivalent of Arg 160 in human SO, is involved in the formation of a positively charged sulfite binding site [Kisker, C., Schindelin, H., Pacheco, A., Wehbi, W., Garnett, R. M., Rajagopalan, K. V., Enemark, J. H., Rees, D. C. (1997) Cell 91, 973-983]. To further assess the role of Arg 160 in human SO, intramolecular electron transfer (IET) rates between the reduced heme [Fe(II)] and oxidized molybdenum [Mo(VI)] centers in the wild type, R160Q, and R160K human SO forms were investigated by laser flash photolysis. In the R160Q mutant, the IET rate constant at pH 6.0 was decreased by nearly 3 orders of magnitude relative to wild type, which indicates that the positive charge of Arg 160 is essential for efficient IET in human SO. Furthermore, the IET rate constant for the R160K mutant is about one-fourth that of the wild type enzyme, which strongly indicates that it is the loss of charge of Arg 160, and not its precise location, that is responsible for the much larger decrease in IET rates in the R160Q mutant. Steady-state kinetic measurements indicate that IET is rate-limiting in the catalytic cycle of the R160Q mutant. Thus, the large decrease in the IET rate constant rationalizes the fatal impact of this mutation in patients with this genetic disorder. 相似文献
5.
Rajapakshe A Meyers KT Berry RE Tollin G Enemark JH 《Journal of biological inorganic chemistry》2012,17(3):345-352
Sulfite oxidase (SO) is a molybdoheme enzyme that is important in sulfur catabolism, and mutations in the active site region
are known to cause SO deficiency disorder in humans. This investigation probes the effects that mutating aromatic residues
(Y273, W338, and H337) in the molybdenum-containing domain of human SO have on both the intramolecular electron transfer (IET)
rate between the molybdenum and iron centers using laser flash photolysis and on catalytic turnover via steady-state kinetic
analysis. The W338 and H337 mutants show large decreases in their IET rate constants (k
ET) relative to the wild-type values, suggesting the importance of these residues for rapid IET. In contrast, these mutants
are catalytically competent and exhibit higher k
cat values than their corresponding k
ET, implying that these two processes involve different conformational states of the protein. Redox potential investigations
using spectroelectrochemistry revealed that these aromatic residues close to the molybdenum center affect the potential of
the presumably distant heme center in the resting state (as shown by the crystal structure of chicken SO), suggesting that
the heme may be interacting with these residues during IET and/or catalytic turnover. These combined results suggest that
in solution human SO may adopt different conformations for IET and for catalysis in the presence of the substrate. For IET
the H337/W338 surface residues may serve as an alternative-docking site for the heme domain. The similarities between the
mutant and wild-type EPR spectra indicate that the active site geometry around the Mo(V) center is not changed by the mutations
studied here. 相似文献
6.
Kayunta Johnson-Winters Amanda C. Davis Anna R. Arnold Robert E. Berry Gordon Tollin John H. Enemark 《Journal of biological inorganic chemistry》2013,18(6):645-653
Sulfite oxidase (SO) is a vital metabolic enzyme that catalyzes the oxidation of toxic sulfite to sulfate. The proposed mechanism of this molybdenum cofactor dependent enzyme involves two one-electron intramolecular electron transfer (IET) steps from the molybdenum center to the iron of the b 5-type heme and two one-electron intermolecular electron transfer steps from the heme to cytochrome c. This work focuses on how the electrostatic interaction between two conserved amino acid residues, R472 and D342, in human SO (hSO) affects catalysis. The hSO variants R472M, R472Q, R472K, R472D, and D342K were created to probe the effect of the position of the salt bridge charges, along with the interaction between these two residues. With the exception of R472K, these variants all showed a significant decrease in their IET rate constants, k et, relative to wild-type hSO, indicating that the salt bridge between residues 472 and 342 is important for rapid IET. Surprisingly, however, except for R472K and R472D, all of the variants show k cat values higher than their corresponding k et values. The turnover number for R472D is about the same as k et, which suggests that the change in this variant is rate-limiting in catalysis. Direct spectroelectrochemical determination of the Fe(III/II) reduction potentials of the heme and calculation of the Mo(VI/V) potentials revealed that all of the variants affected the redox potentials of both metal centers, probably due to changes in their environments. Thus, the position of the positive charge of R472 and that of the negative charge of D342 are both important in hSO, and changing either the position or the nature of these charges perturbs IET and catalysis. 相似文献
7.
Ju-Chun Hsiao Aaron P. McGrath Linda Kielmann Palraj Kalimuthu Farzana Darain Paul V. Bernhardt Jeffrey Harmer Mihwa Lee Kimberley Meyers Megan J. Maher Ulrike Kappler 《BBA》2018,1859(1):19-27
A central conserved arginine, first identified as a clinical mutation leading to sulfite oxidase deficiency, is essential for catalytic competency of sulfite oxidizing molybdoenzymes, but the molecular basis for its effects on turnover and substrate affinity have not been fully elucidated.We have used a bacterial sulfite dehydrogenase, SorT, which lacks an internal heme group, but transfers electrons to an external, electron accepting cytochrome, SorU, to investigate the molecular functions of this arginine residue (Arg78). Assay of the SorT Mo centre catalytic competency in the absence of SorU showed that substitutions in the central arginine (R78Q, R78K and R78M mutations) only moderately altered SorT catalytic properties, except for R78M which caused significant reduction in SorT activity. The substitutions also altered the Mo-centre redox potentials (MoVI/V potential lowered by ca. 60–80 mV). However, all Arg78 mutations significantly impaired the ability of SorT to transfer electrons to SorU, where activities were reduced 17 to 46-fold compared to SorTWT, precluding determination of kinetic parameters. This was accompanied by the observation of conformational changes in both the introduced Gln and Lys residues in the crystal structure of the enzymes. Taking into account data collected by others on related SOE mutations we propose that the formation and maintenance of an electron transfer complex between the Mo centre and electron accepting heme groups is the main function of the central arginine, and that the reduced turnover and increases in KMsulfite are caused by the inefficient operation of the oxidative half reaction of the catalytic cycle in enzymes carrying these mutations. 相似文献
8.
Malin Eh Alexander Tobias Kaczmarek Guenter Schwarz Daniel Bender 《The Journal of biological chemistry》2022,298(3)
Sulfite oxidase (SOX) is a homodimeric molybdoheme enzyme that oxidizes sulfite to sulfate at the molybdenum center. Following substrate oxidation, molybdenum is reduced and subsequently regenerated by two sequential electron transfers (ETs) via heme to cytochrome c. SOX harbors both metals in spatially separated domains within each subunit, suggesting that domain movement is necessary to allow intramolecular ET. To address whether one subunit in a SOX dimer is sufficient for catalysis, we produced heterodimeric SOX variants with abolished sulfite oxidation by replacing the molybdenum-coordinating and essential cysteine in the active site. To further elucidate whether electrons can bifurcate between subunits, we truncated one or both subunits by deleting the heme domain. We generated three SOX heterodimers: (i) SOX/Mo with two active molybdenum centers but one deleted heme domain, (ii) SOX/Mo_C264S with one unmodified and one inactive subunit, and (iii) SOX_C264S/Mo harboring a functional molybdenum center on one subunit and a heme domain on the other subunit. Steady-state kinetics showed 50% SOX activity for the SOX/Mo and SOX/Mo_C264S heterodimers, whereas SOX_C264S/Mo activity was reduced by two orders of magnitude. Rapid reaction kinetics monitoring revealed comparable ET rates in SOX/Mo, SOX/Mo_C264S, and SOX/SOX, whereas in SOX_C264S/Mo, ET was strongly compromised. We also combined a functional SOX Mo domain with an inactive full-length SOX R217W variant and demonstrated interdimer ET that resembled SOX_C264S/Mo activity. Collectively, our results indicate that one functional subunit in SOX is sufficient for catalysis and that electrons derived from either Mo(IV) or Mo(V) follow this path. 相似文献
9.
Identification and biochemical characterization of Arabidopsis thaliana sulfite oxidase. A new player in plant sulfur metabolism 总被引:9,自引:0,他引:9
Eilers T Schwarz G Brinkmann H Witt C Richter T Nieder J Koch B Hille R Hänsch R Mendel RR 《The Journal of biological chemistry》2001,276(50):46989-46994
In mammals and birds, sulfite oxidase (SO) is a homodimeric molybdenum enzyme consisting of an N-terminal heme domain and a C-terminal molybdenum domain (EC ). In plants, the existence of SO has not yet been demonstrated, while sulfite reductase as part of sulfur assimilation is well characterized. Here we report the cloning of a plant sulfite oxidase gene from Arabidopsis thaliana and the biochemical characterization of the encoded protein (At-SO). At-SO is a molybdenum enzyme with molybdopterin as an organic component of the molybdenum cofactor. In contrast to homologous animal enzymes, At-SO lacks the heme domain, which is evident both from the amino acid sequence and from its enzymological and spectral properties. Thus, among eukaryotes, At-SO is the only molybdenum enzyme yet described possessing no redox-active centers other than the molybdenum. UV-visible and EPR spectra as well as apparent K(m) values are presented and compared with the hepatic enzyme. Subcellular analysis of crude cell extracts showed that SO was mostly found in the peroxisomal fraction. In molybdenum cofactor mutants, the activity of SO was strongly reduced. Using antibodies directed against At-SO, we show that a cross-reacting protein of similar size occurs in a wide range of plant species, including both herbacious and woody plants. 相似文献
10.
Wang ZQ Lawson RJ Buddha MR Wei CC Crane BR Munro AW Stuehr DJ 《The Journal of biological chemistry》2007,282(4):2196-2202
Unlike animal nitric-oxide synthases (NOSs), the bacterial NOS enzymes have no attached flavoprotein domain to reduce their heme and so must rely on unknown bacterial proteins for electrons. We tested the ability of two Bacillus subtilis flavodoxins (YkuN and YkuP) to support catalysis by purified B. subtilis NOS (bsNOS). When an NADPH-utilizing bacterial flavodoxin reductase (FLDR) was added to reduce YkuP or YkuN, both supported NO synthesis from either L-arginine or N-hydroxyarginine and supported a linear nitrite accumulation over a 30-min reaction period. Rates of nitrite production were directly dependent on the ratio of YkuN or YkuP to bsNOS. However, the V/Km value for YkuN (5.2 x 10(5)) was about 20 times greater than that of YkuP (2.6 x 10(4)), indicating YkuN is more efficient in supporting bsNOS catalysis. YkuN that was either photo-reduced or prereduced by FLDR transferred an electron to the bsNOS ferric heme at rates similar to those measured for heme reduction in the animal NOSs. YkuN supported a similar NO synthesis activity by a different bacterial NOS (Deinococcus radiodurans) but not by any of the three mammalian NOS oxygenase domains nor by an insect NOS oxygenase domain. Our results establish YkuN as a kinetically competent redox partner for bsNOS and suggest that FLDR/flavodoxin proteins could function physiologically to support catalysis by bacterial NOSs. 相似文献
11.
Kappler U Bailey S Feng C Honeychurch MJ Hanson GR Bernhardt PV Tollin G Enemark JH 《Biochemistry》2006,45(32):9696-9705
The sulfite dehydrogenase from Starkeya novella is the only known sulfite-oxidizing enzyme that forms a permanent heterodimeric complex between a molybdenum and a heme c-containing subunit and can be crystallized in an electron transfer competent conformation. Tyr236 is a highly conserved active site residue in sulfite oxidoreductases and has been shown to interact with a nearby arginine and a molybdenum-oxo ligand that is involved in catalysis. We have created a Tyr236 to Phe substitution in the SorAB sulfite dehydrogenase. The purified SDH(Y236F) protein has been characterized in terms of activity, structure, intramolecular electron transfer, and EPR properties. The substituted protein exhibited reduced turnover rates and substrate affinity as well as an altered reactivity toward molecular oxygen as an electron acceptor. Following reduction by sulfite and unlike SDH(WT), the substituted enzyme was reoxidized quickly in the presence of molecular oxygen, a process reminiscent of the reactions of the sulfite oxidases. SDH(Y236F) also exhibited the pH-dependent CW-EPR signals that are typically observed in vertebrate sulfite oxidases, allowing a direct link of CW-EPR properties to changes caused by a single-amino acid substitution. No quantifiable electron transfer was seen in laser flash photolysis experiments with SDH(Y236F). The crystal structure of SDH(Y236F) clearly shows that as a result of the substitution the hydrogen bonding network surrounding the active site is disturbed, resulting in an increased mobility of the nearby arginine. These disruptions underline the importance of Tyr236 for the integrity of the substrate binding site and the optimal alignment of Arg55, which appears to be necessary for efficient electron transfer. 相似文献
12.
Sulfite oxidase purified from livers of tungsten-treated rats has been used for EPR studies of tungsten substituted at the molybdenum site of the enzyme in a fraction of the molecules. The EPR signal of W(V) in sulfite oxidase is quite similar to that of Mo(V) in its line shape and in its sensitivity to the presence of anions such as phosphate and fluoride. Hyperfine interaction with a dissociable proton is also observed in both signals. The pH-dependent alteration in line shape exhibited by the Mo(V) EPR signal of the rat liver enzyme. Incomplete reduction of the tungsten center at pH 9 is indicated by attenuated signal intensity at this pH. The W(V) signal has g values lower than those of the Mo(V) signal, has a much broader resonance envelope, and is much less readily saturated by increasing microwave power. Kinetic studies on the reduction of the heme and tungsten centers of sulfite oxidase have shown that reduction of de-molybdo forms of sulfite oxidase by sulfite is catalyzed by the residual traces of native molybdenum-containing molecules. Reduction is accomplished by electron transfer involving intermolecular heme-heme interaction. The W(V) signal is generated only after all the heme centers are reduced. The rate and extent of heme reduction at pH 9 are the same as at pH 7. Studies on the reoxidation of W(V) and reduced heme by O2 and by cytochrome c suggest that the cytochrome b5 of sulfite oxidase is the site of electron transfer to cytochrome c, whereas oxidase activity is the property of the molybdenum center. It appears that the tungsten center in sulfite oxidase is incapable of oxidizing sulfite. 相似文献
13.
Astashkin AV Hood BL Feng C Hille R Mendel RR Raitsimring AM Enemark JH 《Biochemistry》2005,44(40):13274-13281
The Mo(V) center of plant sulfite oxidase from Arabidopsis thaliana (At-SO) has been studied by continuous wave and pulsed EPR methods. Three different Mo(V) EPR signals have been observed, depending on pH and the technique used to generate the Mo(V) oxidation state. At pH 6, reduction by sulfite followed by partial reoxidation with ferricyanide generates an EPR spectrum with g-values similar to the low-pH (lpH) form of vertebrate SOs, but no nearby exchangeable protons can be detected. On the other hand, reduction of At-SO with Ti(III) citrate at pH 6 generates a Mo(V) signal with large hyperfine splittings from a single exchangeable proton, as is typically observed for lpH SO from vertebrates. Reduction of At-SO with sulfite at high pH generates the well-known high-pH (hpH) signal common to all sulfite oxidizing enzymes. It is proposed that, depending on the conformation of Arg374, the active site of At-SO may be in "closed" or "open" forms that differ in the degree of accessibility of the Mo center to substrate and water molecules. It is suggested that at low pH the sulfite-reduced At-SO has coordinated sulfate and is in the "closed form". Reoxidation to Mo(V) by ferricyanide leaves bound sulfate trapped at the active site, and consequently, there are no ligands with exchangeable protons. Reduction with Ti(III) citrate injects an electron directly into the active site to generate the [Mo(V)[triple bond]O(OH)]2+ unit that is well-known from model chemistry and which has a single exchangeable proton with a large isotropic hyperfine interaction. At high pH, the active site is in the "open form", and water can readily exchange into the site to generate the hpH SO. 相似文献
14.
Our previous studies have shown that the rate constant for intramolecular electron transfer (IET) between the heme and molybdenum centers of chicken liver sulfite oxidase varies from approximately 20 to 1400 s(-1) depending upon reaction conditions [Pacheco, A., Hazzard, J. T., Tollin, G., and Enemark, J. H. (1999) J. Biol. Inorg. Chem. 4, 390-401]. These two centers are linked by a flexible polypeptide loop, suggesting that conformational changes, which alter the Mo-Fe distance, may play an important role in the observed IET rates. In this study, we have investigated IET in sulfite oxidase using laser flash photolysis as a function of solution viscosity. The solution viscosity was varied over the range of 1.0-2.0 cP by addition of either polyethylene glycol 400 or sucrose. In the presence of either viscosogen, an appreciable decrease in the IET rate constant value is observed with an increase in the solvent viscosity. The IET rate constant exhibits a linear dependence on the negative 0.7th power of the viscosity. Steady-state kinetics and EPR experiments are consistent with the interpretation that viscosity, and not other properties of the added viscosogens, is responsible for the dependence of IET rates on the solvent composition. The results are consistent with the role of conformational changes on IET in sulfite oxidase, which helps to clarify the inconsistency between the large rate constant for IET between the Mo and Fe centers and the long distance (approximately 32 A) between these two metal centers observed in the crystal structure [Kisker, C., Schindelin, H., Pacheco, A., Wehbi, W., Garnett, R. M., Rajagopalan, K. V., Enemark, J. H., and Rees, D. C. (1997) Cell 91, 973-983]. 相似文献
15.
Feng C Tollin G Holliday MA Thomas C Salerno JC Enemark JH Ghosh DK 《Biochemistry》2006,45(20):6354-6362
Intersubunit intraprotein electron transfer (IET) from flavin mononucleotide (FMN) to heme is essential in nitric oxide (NO) synthesis by NO synthase (NOS). Previous crystal structures and functional studies primarily concerned an enzyme conformation, which serves as the input state for reduction of FMN by electrons from NADPH and flavin adenine dinucleotide (FAD) in the reductase domain. To favor the formation of the output state for the subsequent IET from FMN to heme in the oxygenase domain, a novel truncated two-domain oxyFMN construct of rat neuronal NOS (nNOS), in which only the FMN and heme domains were present, was designed and expressed. The kinetics of IET between the FMN and heme domains in the nNOS oxyFMN construct in the presence and absence of added calmodulin (CaM) were directly determined using laser flash photolysis of CO dissociation in comparative studies on partially reduced oxyFMN and single-domain heme oxygenase constructs. The IET rate constant in the presence of CaM (262 s(-)(1)) was increased approximately 10-fold compared to that in the absence of CaM (22 s(-)(1)). The effect of CaM on interdomain interactions was further evidenced by electron paramagnetic resonance (EPR) spectra. This work provides the first direct evidence of the CaM control of electron transfer (ET) between FMN and heme domains through facilitation of the FMN/heme interactions in the output state. Therefore, CaM controls IET between heme and FMN domains by a conformational gated mechanism. This is essential in coupling ET in the reductase domain in NOS with NO synthesis in the oxygenase domain. 相似文献
16.
In the crystal structure of chicken sulfite oxidase, the residue Tyr(322) (Tyr(343) in human sulfite oxidase) was found to directly interact with a bound sulfate molecule and was proposed to have an important role in mediating the substrate specificity and catalytic activity of this molybdoprotein. In order to understand the role of this residue in the catalytic mechanism of sulfite oxidase, steady-state and stopped-flow analyses were performed on wild-type and Y343F human sulfite oxidase over the pH range 6-10. In steady-state assays of Y343F sulfite oxidase using cytochrome c as the electron acceptor, k(cat) was somewhat impaired ( approximately 34% wild-type activity at pH 8.5), whereas the K(m)(sulfite) showed a 5-fold increase over wild type. In rapid kinetic assays of the reductive half-reaction of wild-type human sulfite oxidase, k(red)(heme) changed very little over the entire pH range, with a significant increase in K(d)(sulfite) at high pH. The k(red)(heme) of the Y343F variant was significantly impaired across the entire pH range, and unlike the wild-type protein, both k(red)(heme) and K(d)(sulfite) were dependent on pH, with a significant increase in both kinetic parameters at high pH. Additionally, reduction of the molybdenum center by sulfite was directly measured for the first time in rapid reaction assays using sulfite oxidase lacking the N-terminal heme-containing domain. Reduction of the molybdenum center was quite fast (k(red)(Mo) = 972 s(-1) at pH 8.65 for wild-type protein), indicating that this is not the rate-limiting step in the catalytic cycle. Reduction of the molybdenum center of the Y343F variant by sulfite was more significantly impaired at high pH than at low pH. These results demonstrate that the Tyr(343) residue is important for both substrate binding and oxidation of sulfite by sulfite oxidase. 相似文献
17.
Andrew Pacheco James T. Hazzard G. Tollin J. H. Enemark 《Journal of biological inorganic chemistry》1999,4(4):390-401
The individual rate constants for intramolecular electron transfer (IET) between the MoVIFeII and MoVFeIII forms of chicken liver sulfite oxidase (SO) have been determined at a variety of pH values, and at high and low anion concentrations.
Large anions such as EDTA do not inhibit IET as dramatically as do small anions such as SO4
2– and Cl–, which suggests that specific anion binding at the sterically constrained Mo active site is necessary for IET inhibition
to occur.IET may require that SO adopt a conformation in which the Mo and Fe centers are held in close proximity by electrostatic
interactions between the predominantly positively charged Mo active site, and the negatively charged heme edge. Thus, small
anions which can fit into the Mo active site will weaken this electrostatic attraction and disfavor IET. The rate constant
for IET from FeII to MoVI decreases with increasing pH, both in the presence and absence of 50 mM SO4
2–. However, the rate constant for the reverse process exhibits no significant pH dependence in the absence of SO4
2–, and increases with pH in the presence of 50 mM SO4
2–. This behavior is consistent with a mechanism in which IET from MoV to FeIII is coupled to proton transfer from MoV–OH to OH–, and the reverse IET process is coupled to proton transfer from H2O to MoVI=O. At high concentrations of small anions, direct access of H2O or OH–to the Mo-OH will be blocked, which provides a second possible mechanism for inhibition of IET by such anions. Inhibition
by anions is not strictly competitive, however, and Tyr322 may play an important intermediary role in transferring the proton
when an anion blocks direct access of H2O or OH– to the Mo-OH. Competing H-bonding interactions of the Mo-OH moiety with Tyr322 and with the anion occupying the active site
may also be responsible for the well-known equilibrium between two EPR-distinct forms of SO that is observed for the two-electron
reduced enzyme.
Received: 21 December 1998 / Accepted: 6 April 1999 相似文献
18.
Susan Bailey Trevor Rapson Kayunta Johnson-Winters Andrei V. Astashkin John H. Enemark Ulrike Kappler 《The Journal of biological chemistry》2009,284(4):2053-2063
Sulfite dehydrogenases (SDHs) catalyze the oxidation and detoxification of
sulfite to sulfate, a reaction critical to all forms of life.
Sulfite-oxidizing enzymes contain three conserved active site amino acids
(Arg-55, His-57, and Tyr-236) that are crucial for catalytic competency. Here
we have studied the kinetic and structural effects of two novel and one
previously reported substitution (R55M, H57A, Y236F) in these residues on SDH
catalysis. Both Arg-55 and His-57 were found to have key roles in substrate
binding. An R55M substitution increased
Km(sulfite)(app) by 2–3 orders of
magnitude, whereas His-57 was required for maintaining a high substrate
affinity at low pH when the imidazole ring is fully protonated. This effect
may be mediated by interactions of His-57 with Arg-55 that stabilize the
position of the Arg-55 side chain or, alternatively, may reflect changes in
the protonation state of sulfite. Unlike what is seen for SDHWT and
SDHY236F, the catalytic turnover rates of SDHR55M and
SDHH57A are relatively insensitive to pH (∼60 and 200
s–1, respectively). On the structural level, striking kinetic
effects appeared to correlate with disorder (in SDHH57A and
SDHY236F) or absence of Arg-55 (SDHR55M), suggesting
that Arg-55 and the hydrogen bonding interactions it engages in are crucial
for substrate binding and catalysis. The structure of SDHR55M has
sulfate bound at the active site, a fact that coincides with a significant
increase in the inhibitory effect of sulfate in SDHR55M. Thus,
Arg-55 also appears to be involved in enabling discrimination between the
substrate and product in SDH.Sulfite-oxidizing enzymes protect cells against potentially fatal damage to
DNA and proteins caused by exposure to sulfite, and consequently they are
found in all forms of life (1).
In bacteria, sulfite oxidation is often linked to energy-generating processes
during chemolithotrophic growth on reduced sulfur compounds
(2,
3), whereas both plant and
vertebrate sulfite oxidases have been shown to detoxify sulfite arising from
the degradation of methionine and cysteine and exposure to sulfur dioxide
(4,
5).All known sulfite-oxidizing enzymes belong to the same family of
mononuclear molybdenum enzymes. Their active sites contain one molybdopterin
unit per molybdenum atom, and these enzymes may also contain heme groups as
accessory redox centers
(6–9).
Examples of different types of sulfite-oxidizing molybdoenzymes are the
homodimeric plant sulfite oxidase, which does not contain a heme group and
uses oxygen as its preferred electron acceptor
(9), the homodimeric chicken
and human liver sulfite oxidases
(CSO3 and HSO,
respectively) (10), which are
also able to use oxygen as an electron acceptor, and the bacterial sulfite
dehydrogenase (SDH) isolated from the soil bacterium Starkeya novella
(11,
12), which cannot donate
electrons directly to oxygen. Each monomer of CSO and HSO contains a heme b
center in addition to the molybdenum center, and the redox centers are located
within separate, flexibly linked domains of the same protein subunit. In
contrast, the bacterial enzyme is a heterodimer where each subunit of the
enzyme contains one redox center. The molybdopterin cofactor is located in the
larger 40.2-kDa SorA subunit, and the c-type heme is located in the smaller,
8.8-kDa SorB subunit (12). The
SDH quaternary structure thus differs clearly from that of the human and
chicken sulfite oxidases.Crystal structures are available for plant sulfite oxidase, CSO, and the
bacterial SDH (10,
11,
13–15)
and have revealed molecular details of the sulfite-oxidizing enzymes. In the
CSO structure, the mobile heme b domain occupies a position too removed from
the molybdenum active site to mediate efficient electron transfer
(10), and indeed the kinetics
of this enzyme are known to be complicated by domain movements
(16). In contrast, the
bacterial SDH is a tight complex with strong electrostatic interactions
between the subunits, and the close approach of the redox centers (Mo–Fe
distance 16.6 Å) allows for rapid electron transfer
(11,
17)
(Fig. 1, A and
B).Open in a separate windowFIGURE 1.Details of the crystal structure of wild type SDH and comparison with
CSO. A, ribbon diagram of the SDH heterodimer with the SorA and
SorB subunits colored blue and cyan, respectively, and the
redox cofactors in space-filling mode with the molybdenum atom colored
green and the iron atom colored violet. B, ribbon diagram of a
single subunit of CSO with the molybdopterin binding domain in the same
orientation as SorA in A. The cytochrome domain of CSO is clearly in
a different position with respect to the molybdenum cofactor than is seen for
the cytochrome subunit of SDH. C, SDH molybdopterin cofactor
demonstrating the geometry of the molybdenum ligands. The thiol ligands
donated by the organic component of molybdopterin and the Cys-104 side chain,
and the reactive oxygen ligand (Oeq) sit in the equatorial
plane with the axial oxygen (Oax) ligand at the
apex of a square pyramid. Atoms are colored as
follows: molybdenum (green), sulfur (orange), phosphorous
(magenta), oxygen (red), nitrogen (blue), and carbon
(yellow in the cofactor and white in the protein).
D, hydrogen bonding network around the substrate binding site. The
molybdopterin and heme cofactors are shown together with active site residues
Cys-104, Arg-55, His-57, Tyr-236, and Gln-33. Figs. 1 and
and44 were prepared using Pymol
(37).Despite the overall structural differences of these proteins, the
coordination geometries of the molybdenum active sites of these
sulfite-oxidizing enzymes are nearly identical. The oxidized molybdenum center
has a square pyramidal conformation, with three sulfur and two oxo ligands
(18). Within this molybdenum
center, the equatorial oxo ligand is proposed to be catalytically active,
whereas the axial oxo ligand is not thought to participate directly in the
reaction (Fig. 1C).
During catalysis, the equatorial oxo ligand is transformed into a
hydroxy/water ligand as a result of the reduction of the molybdenum center
(Fig. 2), and it is in this
form that it is generally observed in the CSO and SDH crystal structures.Open in a separate windowFIGURE 2.Proposed reaction mechanism for S. novella sulfite
dehydrogenase. The reaction is shown in terms of the redox states of the
molybdenum and heme centers present in the enzyme. Shown in boldface
type and boxed are the stable redox states of the S.
novella SDH. Cyt. c, a mitochondrial type cytochrome
c550 (e.g. horse heart or S. novella
cytochrome c550) that can act as the external electron
acceptor.SDH, CSO, and HSO show similarly high affinities for their substrate,
sulfite, and several highly conserved residues surround the substrate-binding
and molybdenum active site, namely Tyr-236 (all residues given in SDH
numbering (11)), Arg-55, and
His-57 (Fig. 1D). Both
Arg-55 and Tyr-236 form hydrogen bonds to the catalytically active equatorial
Mo-oxo group, whereas His-57 is positioned close to both Arg-55 and Tyr-236
(10,
11)
(Fig. 1D). In
addition, the crystal structure of the bacterial SDH shows that Arg-55
interacts directly with the second SDH redox center by hydrogen bonding to
heme propionate-6 (Fig.
1D)
(11).As a result of the similarities in catalytic parameters and the structure
of the active site, the bacterial SDH is a very good system for studies of
enzymatic sulfite oxidation and especially the molecular basis for catalysis.
Since this enzyme does not rely on domain movement for catalysis, it has a
less complicated reaction mechanism than the vertebrate enzymes, which
facilitates the interpretation of kinetic data, and it can be readily
crystallized with both redox centers present in an electron transfer competent
conformation. We have previously reported data on the structure, kinetics,
EPR, and redox properties of a Y236F-substituted SDH
(13). In addition to reduced
turnover and substrate affinity, this substitution influences the reactivity
of the SDH toward oxygen, turning SDHY236F essentially into an
(albeit weak) sulfite oxidase. In order to further understand the roles of the
conserved amino acids surrounding the molybdenum active site of
sulfite-oxidizing enzymes, we have created two novel amino acid substitutions
in the Arg-55 and His-57 residues present at the active site and have
investigated their effect on catalytic and spectroscopic parameters of the
bacterial SDH. We have also solved the crystal structures of the substituted
enzymes, which have provided new insights into the conformation and plasticity
of the active site of sulfite-oxidizing enzymes and how the conserved active
site residues contribute to sulfite oxidation. 相似文献
19.
Rate-limiting processes of catalysis by eukaryotic molybdenum-containing nitrate reductase (NaR, EC 1.7.1.1-3) were investigated using two viscosogens (glycerol and sucrose) and observing their impact on NAD(P)H:NaR activity of corn leaf NaR and recombinant Arabidopsis and yeast NaR. Holo-NaR has two "hinge" sequences between stably folded regions housing its internal electron carriers: 1) Hinge 1 between the molybdenum-containing nitrate reducing module and cytochrome b domain containing heme and 2) Hinge 2 between cytochrome b and cytochrome b reductase (CbR) module containing FAD. Solution viscosity negatively impacted the activity of these holo-NaR forms, which suggests that the rate-limiting events in catalysis were likely to involve large conformational changes that restrict or "gate" internal electron-proton transfers (IET). Little effect of viscosity was observed on recombinant CbR module and methyl viologen nitrate reduction by holo-NaR, suggesting that these activities involved no large conformational changes. To determine whether Hinge 2 is involved in gating the first step in IET, the effects of viscosogen on cytochrome c and ferricyanide reductase activities of holo-NaR and ferricyanide reductase activity of the recombinant molybdenum reductase module (CbR, Hinge 2, and cytochrome b) were analyzed. Solution viscosity negatively impacted these partial activities, as if Hinge 2 were involved in gating IET in both enzyme forms. We concluded that both Hinges 1 and 2 appear to be involved in gating IET steps by restricting the movement of the cytochrome b domain relative to the larger nitrate-reducing and electron-donating modules of NaR. 相似文献
20.
The FMN-heme intraprotein electron transfer (IET) kinetics in a human inducible NOS (iNOS) oxygenase/FMN (oxyFMN) construct co-expressed with NCaM, a truncated calmodulin (CaM) construct that includes only its N-terminal globular domain consisting of residues 1-75, were determined by laser flash photolysis. The IET rate constant is significantly decreased by nearly fourfold (compared to the iNOS oxyFMN co-expressed with full length CaM). This supports an important role of full length CaM in proper interdomain FMN/heme alignment in iNOS. The IET process was not observed with added excess EDTA, suggesting that Ca2+ depletion results in the FMN domain moving away from the heme domain. The results indicate that a Ca2+-dependent reorganization of the truncated CaM construct could cause a major modification of the NCaM/iNOS association resulting in a loss of the IET. 相似文献