From the Department of Biochemistry and Molecular
Biology, Nippon Medical School, 1-1-5 Sendagi, Bunkyo-ku, Tokyo
113-0022, Japan, the ¶ Department of Biochemistry, University of
Toronto, Toronto, Ontario M5S1A8, Canada, the
Pharmaceuticals
Development Research Laboratories, Teijin Institute for Bio-Medical
Research, Hino, Tokyo, Japan, the ** Departments of Medical
Biophysics and Molecular and Medical Genetics, University of Toronto,
and the
Ontario Cancer Institute, Princess
Margaret Hospital/University Health Network, Division of
Molecular and Structural Biology, Toronto, Ontario M5G2M9, Canada
Received for publication, August 13, 2002, and in revised form, November 1, 2002
![]() |
ABSTRACT |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
TEI-6720
(2-(3-cyano-4-isobutoxyphenyl)-4-methyl-5-thiazolecarboxylic acid) is
an extremely potent inhibitor of xanthine oxidoreductase. Steady state
kinetics measurements exhibit mixed type inhibition with
Ki and Ki' values of 1.2 ± 0.05 × 10 Xanthine oxidoreductase
(XOR)1 enzymes have been
isolated from a wide range of organisms, from bacteria to man, and they
accelerate the hydroxylation of a wide variety of purine, pyrimidine,
pterin, and aldehyde substrates. All of these proteins have similar
molecular weights and composition of redox centers (1, 2). In humans, the enzyme catalyzes the last two steps of purine catabolism, the
oxidation of hypoxanthine to xanthine and of xanthine to uric acid.
This reaction occurs at a molybdenum-pterin center and from there the
electrons are transferred via two Fe2S2
clusters to the isoalloxazine ring of FAD, which then passes them on to
the second substrate NAD+ (1-5).
XOR is synthesized as xanthine dehydrogenase (XDH; EC 1.1.1.204) with
very low reactivity toward molecular oxygen but high reactivity toward
NAD+ (6, 7). In mammals, however, XDH can easily be
converted to xanthine oxidase (XO; EC 1.1.3.22), which does not
interact with NAD+ but is very efficient in producing
superoxide anion (O Allopurinol (Fig. 1A), an
analogue of hypoxanthine, was developed by Elion et al. (11)
as an XDH inhibitor 30 years ago and has been widely prescribed as a
treatment of hyperuricemia and gout since (12). In addition,
administration of allopurinol has been reported to prevent postischemic
tissue damage by inhibiting XO activity (9). In some cases, however,
severe life-threatening side effects have been reported, such as a
toxicity syndrome dramatized by eosinophila, vasculitits, rash
hepatitis, and progressive renal failure (12). The intrinsic
radical-scavenging features of allopurinol (13) make it difficult to
distinguish between the effects it causes directly and the effects
produced by XOR inhibition, e.g. in the production of
radical species in reperfusion injury.
10 M and 9 ± 0.05 × 10
10 M, respectively.
Fluorescence-monitored titration experiments showed that TEI-6720 bound
very tightly to both the active and the inactive desulfo-form of the
enzyme. The dissociation constant determined for the desulfo-form was
2 ± 0.03 × 10
9 M; for the active
form, the corresponding number was too low to allow accurate
measurements. The crystal structure of the active sulfo-form of milk
xanthine dehydrogenase complexed with TEI-6720 and determined at 2.8-Å
resolution revealed the inhibitor molecule bound in a long, narrow
channel leading to the molybdenum-pterin active site of the enzyme. It
filled up most of the channel and the immediate environment of the
cofactor, very effectively inhibiting the activity of the enzyme
through the prevention of substrate binding. Although the inhibitor did
not directly coordinate to the molybdenum ion, numerous hydrogen bonds
as well as hydrophobic interactions with the protein matrix were
observed, most of which are also used in substrate recognition.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS AND DISCUSSION
CONCLUSIONS
REFERENCES
View larger version (9K):
[in a new window]
Fig. 1.
Chemical structures of allopurinol
(A) and TEI-6720 (B).
As oxypurinol, the oxidation product of allopurinol, is the actual inhibiting species (it coordinates to the reduced molybdenum center of XOR), a lag phase for complete inhibition is to be expected. Once inhibited, the enzyme can also be reactivated by spontaneous reoxidation of the metal cofactor (t1/2 = 300 min at 25 °C) (14). This feature requires the administration of at least three relatively high doses of the drug per day to keep the plasma level of the drug at an effective concentration. Because of these shortcomings, new potent inhibitors, preferentially those with well defined inhibition mechanisms, are still most useful both under clinical and scientific experimental aspects. A potential single-dose, low-concentration regiment would be highly welcomed by patients and physicians but the varied features of inhibition could also provide the biochemically inclined experimentalist with a more refined knowledge of the character of the active site of the enzyme and its exact chemical mechanism (15).
We have undertaken a series of investigations aimed at providing more information about the kinetic and structural properties of recently developed XOR inhibitors. As a first step into this direction, we described the inhibition mechanism of a newly introduced inhibitor, BOF-4272 (sodium-8-(3-methoxy-4-phenylsulfinyl-phenyl) pyrazolo[1,5-a]-1,3,5-triazine-4-olate monohydrate) (16), which has been tested in animal studies and in in vitro experiments as an agent to specifically inhibit XOR-based superoxide generation (17-20).
TEI-6720 (2-(3-cyano-4-isobutoxyphenyl)-4-methyl-5-thiazolecarboxylic
acid) (Fig. 1B) is another recently developed inhibitor of
XOR. When tested in rats and chimpanzees, its inhibition of uric acid
production in vivo was stronger and lasted longer than that
of allopurinol, without causing any noticeable side effects (21, 22).
The molecular structure of this inhibitor is quite dissimilar to that
of substrates like xanthine or hypoxanthine, strongly suggesting that
its mode of action will be different from that of allopurinol. In an
effort to characterize in detail the way TEI-6720 interacts with its
target, we investigated its inhibitory mechanism based on kinetic
measurements and determined the crystal structure of the complex formed
by TEI-6720 with XDH at 2.8-Å resolution.
![]() |
MATERIALS AND METHODS |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Protein Purification-- Bovine milk XO was purified using the method of Ball (23) and the fully active form was obtained by further purification following the procedure described by Nishino et al. (24). XO prepared in this way routinely exhibits an activity:flavin ratio (AFR)2 of 200 at 25 °C indicating that more than 95% of the protein sample is in the active form (24, 25). The XDH form of the enzyme was prepared according to Eger et al. (26). Purified enzyme was stored on ice without freezing in a solution containing 20 mM pyrophosphate buffer (pH 8.5), 40 mM Tris-HCl buffer (pH 7.8), 1 mM salicylate, and 0.2 mM EDTA. The desulfo-form of XO was prepared by incubating the enzyme in storage buffer containing 10 mM KCN for 2 h at 25 °C immediately followed by gel filtration to remove excess cyanide (15). The concentration of XO and XDH was determined by spectrophotometry using a molar extinction coefficient of 37,800 at 450 nm (27). The inhibitor TEI-6720 was provided by Teijin Co., Tokyo, Japan. All other reagents were of the highest purity commercially available.
Preparation of Inhibitor-bound Crystals-- Before crystallization, XDH was passed through a Sephadex G-25 column (Amersham Biosciences AB) to remove salicylate. The eluate was then brought to a concentration of about 75 mg/ml using YM-100 concentrators (Amicon). Crystals could be grown under conditions very similar to the ones described by Eger et al. (26), i.e. crystallization was carried out at 20 °C employing an enzyme concentration of 7.5 mg/ml in a solution containing 50 mM potassium phosphate buffer (pH 6.5), 5 mM dithiothreitol, 1 mM salicylate, 0.2 mM EDTA, 30% glycerol, 0.5 mM TEI-6720 as well as 6-10% (w/v) PEG 4,000 as precipitant.
Data Collection-- Crystals of the enzyme-inhibitor complex were flash-frozen with their mother liquor as cryoprotectant and mounted in cryoloops. Diffraction data were collected at beamline BL40B2, SPring8, Harima Garden City, Japan; a temperature of 100 K, radiation of 1.00 Å wavelength, and a Q4 area detector (ACSD) were used. Data were reduced with the help of the program package DENZO and scaled using SCALEPACK (28).
Structure Determination-- The program package EPMR (29) established the correct solutions of the respective molecular replacement function (20.0 to 4.0-Å resolution range). One subunit of bovine milk XDH (Protein Data Bank code 1FO4) without its cofactors was employed as the search model. The molecular models were built with the help of the program package O (30). Subsequent refinement, including rigid body, simulated annealing, grouped B factors, and least square minimization were carried out with CNS, version 1.0 (31). The R-free reflection set was chosen in random resolution shells using the DATAMAN program from CCP4 (32). No NCS constraints were used in the final round of refinement (Table I). Figures were generated with MOLSCRIPT (33) and RASTER3D (34).
|
Enzyme Assay-- Xanthine oxidase activity was determined by following the rate of uric acid formation at 295 nm. Assays were performed in solutions of 0.15 mM xanthine and 0.2 mM EDTA in 0.1 M pyrophosphate buffer (pH 8.5) under air-saturated conditions at 25 °C (26). Xanthine-phenazine methosulfate (PMS) activity was measured by following the PMS-linked reduction of horse heart cytochrome c (Roche Molecular Biochemicals) (35). The reduction of cytochrome c was determined by monitoring the absorbance change at 550 nm in 0.1 M pyrophosphate buffer (pH 8.5) containing 0.2 mM EDTA, 0.15 mM xanthine, 16.7 µM PMS, and 16.7 µM cytochrome c at 25 °C. The PMS solution was kept on ice and in the dark before use. As TEI-6720 exhibits time-dependent inhibition, enzyme activities were determined not from initial rates but from the steady state rates after absorbance changes had sufficiently stabilized.
Determination of Dissociation Constants--
Dissociation
constants (Kd value) for enzyme-inhibitor complexes
were determined by titrating the enzyme with TEI-6720. The mixture was
incubated for 10 min in the dark at 25 °C to ensure equilibrium
before the fluorescence (excitation at 314 nm and emission at 390 nm)
of the solution was measured. As previously described (16),
Kd values were calculated from the plots of
fluorescence versus the total concentrations of added inhibitor.
![]() |
RESULTS AND DISCUSSION |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Time Course of TEI-6720 Inhibition--
As is commonly observed in
tight-binding inhibitors (36), both allopurinol and TEI-6720 show
time-dependent inhibition (Fig. 2). The underlying reasons for their time
dependence, however, are quite different. A relatively large excess of
3.3 µM allopurinol reduced the rate gradually until
complete inactivation was achieved; in contrast, a slight excess of 33 nM TEI-6720 caused a progressive rate decline and finally
reached a steady state level of catalytic activity. Massey et
al. (15) have studied the mechanism of allopurinol inhibition of
XOR in detail. They found that the enzyme oxidizes allopurinol to
oxypurinol, which then in turn coordinates tightly to the pterin-bound
Mo(IV) ion, preventing further catalysis. As a result, the enzyme
activity decreases in proportion to the accumulation of the
oxypurinol-Mo(IV) complex, a classical example of suicide inhibition.
Crystal structures of the oxypurinol complexes of bacterial (37) and
bovine XDH3 show this
inhibitor replaces the hydroxyl ligand of the molybdenum ion.
|
TEI-6720, as recovered from its XOR complex, was chemically unchanged, no hydroxylation had occurred (data not shown). Therefore, we interpret the time dependence of the inhibition as caused by multiple steps for the finally settled enzyme-inhibitor complex after initial binding of the inhibitor, a process rather commonly observed in the formation of such tight binding. No hydroxylation during binding is consistent with the fact that no coordination to the metal cofactor was observed in the crystal structure of the XDH·TEI-6720 complex discussed below.
Steady State Kinetics--
The coexistence of inhibitory effects
caused by TEI-6720 and product inhibition by NADH (38) conspired to
prevent a meaningful steady state analysis of XDH activity. As the
Mo-pterin sites of both XDH and XO are structurally equivalent (10),
steady state kinetics of the product inhibition-free oxidase reaction were measured instead. These analyses were performed varying the concentrations of xanthine and TEI-6720 under air-saturated conditions. A representative Lineweaver-Burk plot is given in Fig.
3. As described for BOF-4272 (16),
TEI-6720 exhibits mixed-type inhibition. Binding of TEI-6720 to the
active enzyme was too tight to allow concentrations of free inhibitor
(Ifree) to be set equal to the initial concentrations of
TEI-6720 (I0). In the inset, concentrations of
free TEI-6720 were corrected according to Equations 1 and 2 (16,
36).
|
![]() |
(Eq. 1) |
![]() |
(Eq. 2) |
|
When catalyzing the transfer of electrons from xanthine to oxygen as the terminal acceptor, XO applies a ping-pong mechanism alternating the positive charge of molybdenum between Mo(VI) and Mo(IV) (27, 39). However, when PMS is used as an electron acceptor, it very rapidly oxidizes Mo(IV), not allowing the collection of meaningful information about this state during turnover. The same is true in the case of allopurinol and BOF-4272 inhibition (15, 16, 40), suggesting that the inhibitor-Mo(VI) complex is the main molecular species formed and represented in a competitive inhibition pattern in Fig. 4. As the Ki value determined for the xanthine oxidase activity (estimated by plotting the slopes in the secondary plot) is almost identical to the one found for xanthine-PMS activity, these values would be representative for the Mo(VI) state of the enzyme, whereas the Ki' value for the xanthine oxidase activity, the same as the one established for BOF-4272 (16), would refer to the Mo(IV) state.
Spectral Perturbation upon Inhibitor Binding--
When fully
active XO was titrated with TEI-6720 (Fig.
5A), significant spectral
perturbations were observed in the UV and visible regions of the
spectrum. The difference spectrum exhibited two negative peaks; the
larger one at 400 nm ( = 1.3 × 103
M
1 cm
1) and a rather shallow,
ill-defined one centered at 550 nm. Their amplitudes increased in
proportion to the amount of inhibitor added until the inhibitor
concentration reached that of the enzyme, which indicated that the
formation of the inhibitor-enzyme complex was causing the spectral
perturbation. However, both the spectral difference and the
dissociation constant were too small to allow the direct determination
of the Kd value from a spectral titration
experiment.
|
If, however, desulfo-XO was used in the titration experiment, no absorption changes were recorded (Fig. 5B) despite the facile formation of a tight-inhibitor complex. The absorbance changes described above are different from those Ryan et al. (41) assigned to the change of the redox state of the molybdenum ion.
Quenching of TEI-6720 Fluorescence upon Enzyme Binding--
Upon
the formation of the enzyme complex, the fluorescence of TEI-6720 with
a peak at 390 nm (excitation at 319 nm) is quenched. We used this
property to measure the dissociation constants of the TEI-6720·XO
complexes of both desulfo-XO (AFR = 3) and fully active XO
(AFR = 190). A plot of fluorescence intensity against the TEI-6720
concentration is given in Fig. 6. The
fluorescence signal increased markedly after equimolar amounts of
TEI-6720 had been added to the enzyme solution, implying a 1:1 ratio of TEI-6720 to enzyme in the complex and making a single, specific binding
site of the inhibitor on the enzyme very plausible. The Kd value for TEI-6720 binding to desulfo-XO was
calculated as 2 ± 0.03 × 109 M.
Again, the corresponding value for the fully active enzyme could not be
determined because the combination of very tight binding by the
inhibitor and rather low fluorescence intensity prevented the
sufficiently accurate determination of the concentration of free
inhibitor (Fig. 6, inset). Given the very small structural difference between the sulfo- and desulfo-forms of the enzyme (replacement of a sulfur atom by an oxygen), one might expect the
interactions between the inhibitor molecule and the protein matrix to
stay the same in the two forms of the enzyme. The distinctive spectral
changes together with the difference in Kd values between the respective TEI-6720 complexes, however, seem to reflect subtle differences in the local electrostatic fields and/or minor structural rearrangements that occur around the molybdenum ion when the
active sulfo-form of the enzyme is transformed into the inactive
desulfo-form.
|
Crystal Structure of the Enzyme-Inhibitor Complex--
Freshly
purified XDH produced crystals in space group C2 with unit cell axes
a = 168.3 Å, b = 124.6 Å,
c = 147.3 Å, and = 91.0°. These parameters
correspond closely to those of the free or salicylate-bound crystals of
XDH (26). The crystals diffracted to 2.8-Å resolution and contained
two subunits in the asymmetric unit.
The overall structure of the protein chain in the inhibitor complex was
identical to the one found in the salicylate-bound enzyme (10). Clear
electron density representing the bound TEI-6720 molecule was
identified and easily interpreted (Fig.
7). TEI-6720 bound in the channel leading
from bulk solvent to the buried Mo-pterin cofactor, closing it off like
a plug. With a distance of 4.9 Å, the methyl carbon in the thiazole
ring was the atom closest to the molybdenum ion. However, no electron
density representing a potential covalent bond between TEI-6720 and
molybdenum was observed. The torsion angle between the planes of the
thiazole and benzonitrile rings was 30°.
|
Six hydrogen bonds and one charge-charge interaction were observed between TEI-6720 and the protein. The most tightly bound part of the inhibitor molecule was its carboxylate group. It was located at almost the same position as the carboxylate group of the salicylate molecule in the original XDH crystal structure (10) and displayed an identical binding pattern: its oxygen atoms interacted with the side chain guanidinium group of Arg880 and, in addition, one of them formed hydrogen bonds to the side chain hydroxyl and the backbone amide of Thr1010. Although the interactions between protein and inhibitor that involve the carboxylate group of the latter strongly contributed to the formation of the tight complex, there had to exist other interactions to explain the 106-fold difference between the Ki values of TEI-6720 and salicylate. Indeed, several such interactions could be identified. The side chain amide of Asn768 and the nitrile group of TEI-6720 were 2.9 Å apart. In addition to providing binding energy, this interaction could be essential in stabilizing the position of the benzene ring. When the 3-cyano moiety of TEI-6720 was replaced by hydrogen, its binding affinity was significantly decreased. In contrast, when the CN-group of the inhibitor was substituted with a nitro ligand, which is also capable of accepting a hydrogen bond, the resulting derivative showed a binding affinity very similar to that of TEI-6720.4
The carboxylate group of Glu802 was located 2.8 Å from N-3 of the thiazole ring. Given this distance and pKa values of 2.5 and 4.6 for thiazole and the side chain of glutamate, respectively, the most probable scenario has the binding of the inhibitor causing the protonation of Glu802 and the formation of a hydrogen bond between the thiazole nitrogen and the carboxylate side chain. The hydrophobic character of large parts of the TEI-6270-binding channel would favor a shift of the pKa value of glutamate in the required direction.
The thiazole ring as a whole was sandwiched between two phenylalanine
residues, Phe914 and Phe1009 (Fig.
8A). The aromatic ring of
Phe914 lay parallel to the plane of the thiazole ring at a
distance of 3.4 Å, whereas the side chain of Phe1009
pointed perpendicularly to the center of the thiazole ring, approaching it to 4.0 Å. This arrangement of energetically favorable
aromatic/aromatic interactions (42) had also been seen in the crystal
structure of the salicylate complex and its conservation argues for an
important role in stabilizing the binding positions of aromatic
substrates; it might well represent one of the key features of
substrate recognition.
|
Hydrophobic interactions also contributed to the binding of TEI-6720 to XOR. The benzonitrile portion of TEI was inserted between Leu873 and Leu1014, keeping a distance of 3.4 and 3.7 Å from each side chains. Together with the Asn768-nitrile bond, this arrangement guides the orientation of the benzonitrile part of the inhibitor. The hydrophobic 4-isobutoxy tail of TEI-6720 was surrounded by amino acids Leu648, Phe649, Val1011, and Leu1013, with distances ranging from 3.7 to 4.2 Å (Fig. 8A). Although some of these crystallographically determined values are too large to argue for direct van der Waals binding, they establish a pocket well suited to accommodate bulky hydrophobic moieties, which are often found as part of the molecular structures of good substrates or inhibitors of XOR (16, 43). The numerous interactions, which the TEI-6720 molecule displayed when assuming its position in the elongated access channel leading to the Mo-pterin group, are illustrated in Fig. 8B. The space filling representation conveys the generally very tight fit between the inhibitor molecule and surrounding residues.
Almost all amino acids, whose interactions with the TEI-6720 molecule are discussed above, are conserved among bovine (44) and human XOR (45). The only exceptions are Leu648 and Phe649 (bovine XOR), which are Ile and Cys in human XOR, respectively. This change still preserves the hydrophobic character of the side chains, the property important in their interaction with the inhibitor molecule. Therefore, the mechanistic conclusions drawn in our discussion are fully applicable to the human enzyme as well.
Correlation of Spectroscopic and Structural Results in the TEI-6720 Complex of XOR-- TEI-6720 bound more tightly to the sulfo-form than to the desulfo-form of XOR (16) and only in the case of the catalytically competent sulfo-form were spectral perturbations observed. The display of biphasic inhibition kinetics was probably caused by two binding modes of the inhibitor (e.g. 1, attached to the channel entrance and 2, fully inserted) and not by structural rearrangements of the accommodating binding site, as there were no overall changes observed in the location and orientation of the protein matrix when TEI-6720 was bound to XOR. In the crystal structure, the methyl substituent of the thiazole ring represented the part of the inhibitor closest to the molybdenum complex approaching its hydroxy ligand to a distance of 3.5 Å. The oxygen atom of the latter has been proposed as the one incorporated into substrate molecules (46). However, an analogous compound, in which the methyl moiety of TEI-6720 has been removed, will also perturb the spectrum in a way very similar to TEI-6720,5 effectively ruling out this interaction as the source of spectral variation.
As the spectral changes are only observed in the sulfo-form, it is interesting to note that the shortest distance between the sulfur ligand of Mo-pterin and the TEI-6720 molecule was 5.0 Å, again making it very improbable that the reason for the modified absorption behavior would be a direct influence by the inhibitor on the sulfur ligand of the cofactor. Although a crystal structure of the desulfo-form of XOR is not yet available, the structure of the salicylate-bound form of bovine XDH (10) supported by the recent results of a 1.7-Å resolution refinement3 can serve as comparison because its absorption spectrum is identical to the one displayed by the desulfo-form, not showing the conspicuous changes in the 400-500 nm region.
The only significant difference found was the movement of the side
chain of Glu802. Above, we have discussed the potential of
this side chain to undergo protonation and to engage in a hydrogen bond
with the N-3 atom of the thiazole ring. On the other hand, in the
salicylate-bound form, Glu802 is 3.3 Å apart from the
sulfur ligand and likely to have a hydrogen bond to the sulfur (10). We
believe that such a change in charge close to the sulfur ligand
combined with an increase in distance between these groups, at the
moment represents the best explanation of how inhibitor binding can
influence the electronic structure of the Mo-pterin cofactor.
![]() |
CONCLUSIONS |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
The crystal structure of the TEI-6720 complex of bovine XOR showed the inhibitor bound in a narrow channel leading to the molybdenum center of the enzyme. The potential drug molecule fills the entire pocket thereby inhibiting the activity of the enzyme simply by obstructing substrate binding. Although no direct coordination was observed between the molybdenum ion and the inhibitor, numerous hydrogen bonds and hydrophobic interactions are evident, some of them conserved in their contribution to substrate recognition. A slight reorientation of a glutamate side chain, probably accompanied by its protonation, is postulated to be the cause of the spectral changes observed upon binding of TEI-6720 to the sulfo-form of XOR.
In stark contrast to oxypurinol, the metabolite of the standard
anti-gout drug allopurinol, which is the actual inhibitor of XOR
activity in vivo and binds tightly only to the reduced form
of the enzyme, TEI-6720 forms very strong complexes with both Mo(VI)
(Ki = 1.2 ± 0.05 × 1010
M) and Mo(IV) forms (Ki' = 9 ± 0.05 × 10
10 M) of XOR. In addition,
oxypurinol-inhibited enzyme is reactivated relatively quickly
(t1/2 = 300 min at 25 °C) by spontaneous
reoxidation of the molybdenum cofactor (15). TEI-6720, however, would
be expected to inhibit the enzyme in vivo for long periods
of time, because the enzyme-inhibitor complex is very stable and not
influenced by changes in the redox status of the cofactor. These
differences between the two XOR inhibitors should translate into
obvious therapeutic advantages for TEI-6720 enabling treatment of
patients with a single daily dose at significantly lower and more
constant plasma concentration levels of the drug. As a pure research
tool, an inhibitor like TEI-6720 will provide the opportunity to
selectively evaluate the contribution of XOR activity to pathogenesis
in effects such as postischemic reperfusion injury, independent of the
metabolic state of the tissue investigated.
![]() |
ACKNOWLEDGEMENTS |
---|
We thank SPring8 for beamtime and Dr. K. Miura for help with data collection.
![]() |
FOOTNOTES |
---|
* This work was supported by Grants-in-aid 11169231 and 12147208 (to T. N.) for Science Research on Priority Areas, Grant-in-aid 13480212 (to T. N.) for Science Research from the Ministry of Education, Science, Sports and Culture of Japan, and a grant from the Canadian Institutes of Health Research, Institute of Genetics (to E. F. P.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
The atomic coordinates and the structure factors (code 1N5X) have been deposited in the Protein Data Bank, Research Collaboratory for Structural Bioinformatics, Rutgers University, New Brunswick, NJ (http://www.rcsb.org/).
§ Both authors contributed equally to the results of this article.
§§ To whom correspondence and reprint requests may be addressed. E-mail: pai@hera.med.utoronto.ca.
¶¶ To whom correspondence and reprint requests may be addressed. E-mail: nishino@nms.ac.jp.
Published, JBC Papers in Press, November 5, 2002, DOI 10.1074/jbc.M208307200
2 AFR is enzyme activity defined as the absorbance change/min at 295 nm (monitoring conversion of xanthine to uric acid) divided by the enzyme absorbance at 450 nm under standard assay conditions.
3 B. T. Eger, K. Okamoto, T. Nishino, T. Nishino, and E. F. Pai, unpublished results.
4 S. Kondo, unpublished results.
5 K. Okamoto, unpublished observations.
![]() |
ABBREVIATIONS |
---|
The abbreviations used are: XOR, xanthine oxidoreductase; XDH, xanthine dehydrogenase; XO, xanthine oxidase; TEI-67620, 2-(3-cyano-4-isobutoxyphenyl)-4-methyl-5-thiazolecarboxylic acid; BOF-4272, sodium-8-(3-methoxy-4-phenylsulfonylphenyl)pyrazolo[1,5-a]-1,3,5-triazine-4-olate monohydrate; AFR, activity to flavin ratio; PMS, phenazine methosulfate; Mo-pterin, molybdenum-pterin.
![]() |
REFERENCES |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
1. | Nishino, T. (1994) J. Biochem. (Tokyo) 116, 1-6[Abstract] |
2. |
Hille, R.,
and Nishino, T.
(1995)
FASEB J.
9,
995-1003 |
3. | Bray, R. C. (1975) in The Enzymes XII (Boyer, P. D., ed) , pp. 300-419, Academic Press, New York |
4. | Hille, R., and Massey, V. (1985) in Molybdenum Enzymes (Spiro, T. G., ed), Vol. 7 , pp. 443-518, Wiley Interscience, New York |
5. | Hille, R. (1996) Chem. Rev. 96, 2757-2816[CrossRef][Medline] [Order article via Infotrieve] |
6. | Stirpe, F., and Della Corte, E. (1969) J. Biol. Chem. 244, 3855-3863[Medline] [Order article via Infotrieve] |
7. | Della Corte, E., and Stirpe, F. (1972) Biochem. J. 126, 739-745[Medline] [Order article via Infotrieve] |
8. |
Nishino, T.,
and Nishino, T.
(1997)
J. Biol. Chem.
272,
29859-29864 |
9. | McCord, J. M. (1985) N. Engl. J. Med. 312, 159-163[Abstract] |
10. |
Enroth, C.,
Eger, B. T.,
Okamoto, K.,
Nishino, T.,
and Pai, E. F.
(2000)
Proc. Natl. Acad. Sci. U. S. A.
97,
10723-10728 |
11. | Elion, G. B., Callahan, S., Nathan, H., Bieber, S., Rundles, R. W., and Hitching, G. H. (1963) Biochem. Pharmacol. 12, 85-93[CrossRef] |
12. | Reginato, A. J. (2001) in Harrison's Principles of Internal Medicine (Braunwald, E., ed), 15th Ed. , pp. 1994-1998, McGraw-Hill, Columbus, OH |
13. | Moorhouse, P. C., Grootveld, M., Halliwell, B., Quinlan, J. G., and Gutteridge, J. M. C. (1987) FEBS Lett. 213, 23-28[CrossRef][Medline] [Order article via Infotrieve] |
14. |
Massey, V.,
Komai, H.,
Palmer, G.,
and Elion, G. B.
(1970)
J. Biol. Chem.
245,
2837-2844 |
15. |
Massey, V.,
and Edmondson, D.
(1970)
J. Biol. Chem.
245,
6595-6598 |
16. |
Okamoto, K.,
and Nishino, T.
(1995)
J. Biol. Chem.
270,
7816-7821 |
17. | Sanders, S. A., Eisenthal, R., and Harrison, R. (1997) Eur. J. Biochem. 245, 541-548[Abstract] |
18. | Matsumura, F., Yamaguchi, Y., Goto, M., Ichiguchi, O., Akizuki, E., Matsuda, T., Okabe, K., Liang, J., Ohshiro, H., Iwamoto, T., Yamada, S., Mori, K., and Ogawa, M. (1998) Hepatology 28, 1578-1587[Medline] [Order article via Infotrieve] |
19. | Millar, T. M., Stevens, C. R., Benjamin, N., Eisenthal, R., Harrison, R., and Blake, D. R. (1998) FEBS Lett. 427, 225-228[CrossRef][Medline] [Order article via Infotrieve] |
20. |
Suzuki, H.,
DeLano, F. A.,
Parks, D. A.,
Jamshidi, N.,
Granger, D. N.,
Ishii, H.,
Suematsu, M.,
Zweifach, B. W.,
and Schmid-Schonbein, G. W.
(1998)
Proc. Natl. Acad. Sci. U. S. A.
95,
4754-4759 |
21. | Osada, Y., Tsuchimoto, M., Fukushima, H., Takahashi, K., Kondo, S., Hasegawa, M., and Komoriya, K. (1993) Eur. J. Pharmacol. 241, 183-188[CrossRef][Medline] [Order article via Infotrieve] |
22. | Komoriya, K., Osada, Y., Hasegawa, M., Horiuchi, H., Kondo, S., Couch, R. C., and Griffin, T. B. (1993) Eur. J. Pharmacol. 250, 455-460[CrossRef][Medline] [Order article via Infotrieve] |
23. | Ball, E. G. (1939) J. Biol. Chem. 128, 51-67 |
24. | Nishino, T., Nishino, T., and Tsushima, K. (1981) FEBS Lett. 131, 369-372[CrossRef][Medline] [Order article via Infotrieve] |
25. | Massey, V., Komai, H., Palmer, G., and Elion, G. B. (1970) Vitam. Horm. 28, 505-531[Medline] [Order article via Infotrieve] |
26. | Eger, B. T., Okamoto, K., Enroth, C., Sato, M., Nishino, T., Pai, E. F., and Nishino, T. (2000) Acta Crystallogr. Sect. D Biol. Crystallogr. 56, 1656-1658[CrossRef][Medline] [Order article via Infotrieve] |
27. |
Massey, V.,
Brumby, P. E.,
and Komai, H.
(1969)
J. Biol. Chem.
244,
1682-1691 |
28. | Otwinoski, Z., and Minor, W. (1997) Methods Enzymol. 276, 307-326 |
29. | Kissinger, C. R., Gehlhaar, D. K., and Fogel, D. B. (1999) Acta Crystallogr. Sect. D Biol. Crystallogr. 55, 484-491[CrossRef][Medline] [Order article via Infotrieve] |
30. | Jones, T. A., Zou, J. Y., Cowan, S. W., and Kjeldgaard, M. (1991) Acta Crystallogr. Sect. A 47, 110-119[CrossRef][Medline] [Order article via Infotrieve] |
31. | Brunger, A. T., Adams, P. D., Clore, G. M., DeLano, W. L., Gros, P., Grosse-Kunstleve, R. W., Jiang, J. S., Kuszewski, J., Nilges, M., Pannu, N. S., Read, R. J., Rice, L. M., Simonson, T., and Warren, G. L. (1998) Acta Crystallogr. D Biol. Crystallogr. 54, 905-921[CrossRef][Medline] [Order article via Infotrieve] |
32. | Kleywegt, G. J., and Jones, T. A. (1996) Acta Crystallogr. D Biol. Crystallogr. 52, 826-828[CrossRef] |
33. | Kraulis, P. (1991) J. Appl. Crystallogr. 24, 946-950[CrossRef] |
34. | Merritt, E. A., and Bacon, D. J. (1997) Methods Enzymol. 277, 505-524 |
35. |
Nishino, T.,
Tsushima, K.,
Hille, R.,
and Massey, V.
(1982)
J. Biol. Chem.
257,
7348-7353 |
36. | Cha, S. (1975) Biochem. Pharmacol. 24, 2177-2185[CrossRef][Medline] [Order article via Infotrieve] |
37. | Truglio, J. J., Theis, K., Leimkuhler, S., Rappa, R., Rajagopalan, K. V., and Kisker, C. (2002) Structure (Lond.) 1, 115-125[CrossRef] |
38. | Della Corte, E., and Stirpe, F. (1970) Biochem. J. 117, 97-100[Medline] [Order article via Infotrieve] |
39. |
Olson, J. S.,
Ballow, D. P.,
Palmer, G.,
and Massey, V.
(1974)
J. Biol. Chem.
249,
4350-4362 |
40. | Spector, T., and Johns, D. G. (1968) Biochem. Biophys. Res. Commun. 32, 1039-1044[Medline] [Order article via Infotrieve] |
41. |
Ryan, M. G.,
Ratnam, K.,
and Hille, R.
(1995)
J. Biol. Chem.
270,
19209-19212 |
42. | Burley, S. K., and Petsko, G. A. (1985) Science 229, 23-28[Medline] [Order article via Infotrieve] |
43. | Beedham, C. (1987) in Progress in Medical Chemistry (Ellis, G. P. , and West, G. B., eds), Vol. 24 , pp. 85-127, Elsevier, Amsterdam |
44. |
Berglund, L.,
Rasmussen, J. T.,
Andersen, M. D.,
Rasmussen, M. S.,
and Petersen, T. E.
(1996)
J. Dairy Sci.
79,
198-204 |
45. | Ichida, K., Amaya, Y., Noda, K., Minoshima, S., Hosoya, T., Sakai, O., Shimizu, N., and Nishino, T. (1993) Gene (Amst.) 133, 279-284[CrossRef][Medline] [Order article via Infotrieve] |
46. |
Xia, M.,
Dempski, R.,
and Hille, R.
(1999)
J. Biol. Chem.
274,
3323-3330 |