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1 Hefei National Laboratory for Physical Sciences at Microscale and School of Life Sciences, University of Science & Technology of China, Hefei, Anhui 230027, China
2 Key Laboratory of Structural Biology, Chinese Academy of Sciences, Hefei, Anhui 230027, China
3 MacCHESS, Cornell High Energy Synchrotron Source, Cornell University, Ithaca, New York 14853, USA
(RECEIVED November 13, 2005; FINAL REVISION December 7, 2005; ACCEPTED December 13, 2005)
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-helix domain. Examination of the structure reveals the participation of a series of residues in catalysis different from other extradiol dioxygenases. Together with two iron-binding residues (His49 and Glu55), Asp120, Asn51, Glu111, and Arg114 form a hydrogen-bonding network; this hydrogen-bond network is key to the catalysis of 3HAO. Residues Arg101, Gln59, and the substrate-binding hydrophobic pocket are crucial for substrate specificity. Structure comparison with 3HAO from Ralstonia metallidurans reveals similarities at the active site and suggests the same catalytic mechanism in prokaryotic and eukaryotic 3HAO. Based on sequence comparison, we suggest that bicupin of human 3HAO is the first example of evolution from a monocupin dimer to bicupin monomer in the diverse cupin superfamilies. Based on the model of the substrate HAA at the active site of Y3HAO, we propose a mechanism of catalysis for 3HAO. Keywords: X-ray crystallography; kynurenine pathway; extradiol dioxygenase; cupin superfamily; 2-His-1-carboxylate facial triad; MAD; 3-hydroxyanthranilic acid 3,4-dioxygenase
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-amino--carboxymuconic 
-semialdehyde is then nonenzymatically transformed to QUIN, which is the source of much of the nicotinic acid required physiologically for the synthesis of nicotinamide and the essential enzymatic cofactors such as nicotinamide adenine dinucleotide (NAD+) (Schwarcz and Pellicciari 2002; Nandi et al. 2003). Interest in the importance of this pathway was aroused with the discovery that it includes several compounds relevant to neurodegeneration and inflammatory neurological diseases (Heyes et al. 1996); 3-hydroxykynurenine and HAA can produce neuronal damage, primarily by the induction of free radical formation (Schwarcz and Pellicciari 2002; Stone and Darlington 2002). Kynurenic acid was shown to be an antagonist at NMDA, kainite, and -amino-3-hydroxy-5-methyl-isoxazole (AMPA) receptors, whereas QUIN proved to excite neurons via the activation of NMDA receptors, and consequently produced neuronal damage (Schwarcz et al. 1983). Hyperactivity of 3HAO has been implicated as a damaging defect in Huntington's disease (Schwarcz et al. 1988; Guidetti et al. 2004), and the neurotoxic capacity of QUIN in vivo has also implicated it in a variety of other neurodegenerative disorders, including epilepsy, Alzheimer's disease, and AIDS dementia complex (Heyes et al. 1992). Manipulation of the kynurenine pathway of tryptophan metabolism, such as inhibition of the activity of the enzymes responsible for synthesizing QUIN, has yielded a plethora of agents that are now being developed as neuroprotectants and anticonvulsants (Schwarcz and Pellicciari 2002; Stone and Darlington 2002). Most of the enzymes in the kynurenine pathway have been identified in humans and in yeast. Enzymatic properties of 3HAO purified from many mammalian tissues, such as beef liver, beef kidney, rat liver, and rat brain, have been extensively studied since 1962 (Nandi et al. 2003). Recently the similar tryptophan-to-QUIN pathway has been discovered in several bacterial species (Kurnasov et al. 2003), and a novel 2-nitrobenzoate degradation pathway by the formation of HAA as an intermediate has also been revealed in Pseudomonas fluorescens strain KU-7A and Arthrobacter protophormiae RKJ100 (Hasegawa et al. 2000; Pandey et al. 2003). The prokaryotic 3HAO enzymes show apparent homology with the eukaryotic ones (Muraki et al. 2003).
3HAO belongs to the type III non-heme ferrous extradiol dioxygenases. Extradiol dioxygenases are divided into at least three evolutionary independent families: Type I extradiol dioxygenases belong to the vicinal oxygen chelate superfamily. These include one-domain enzymes, such as the 2,3-dihydroxybiphenyl 1,2-dioxygenases II and III from Rhodococcus globerulus P6, and two-do-main enzymes, such as the 2,3-dihydroxybiphenyl 1,2-dioxygenase from Pseudomonas sp. strain KKS102, which correspond to Class I and Class II dioxygenases according to Spence et al. (1996). Type II extradiol dioxygenases are multimers, such as Protocatechuate 4,5-dioxygenase(LigAB) from Sphingomonas paucimobilis SYK-6. Type III extradiol dioxygenases belong to the cupin super-family and include enzymes such as the gentisate, homogentisate dioxygenases, 1-hydroxy-2-naphthoate dioxygenase, and 3HAO (Vetting et al. 2004; Nogales et al. 2005).
The typical catechol extradiol dioxygenases play important environmental roles by facilitating the aerobic degradation of catechol derivatives by soil bacteria (Solomon et al. 2000). Although catecholic extradiol dioxygenases utilize Fe2+ to cleave a bond located adjacent to only one of the ortho-hydroxyl groups, and 3HAO cleaves a bond located adjacent to the hydroxyl group of 3-hydroxyanthranilate, the region believed to be important for iron binding is highly conserved (Bugg et al. 1997). All of these enzymes contain one non-heme Fe2+ and cleave aromatic substrates using dioxygen with no other cosubstrates and cofactors. The mechanism of 3HAO was deduced to be similar to the proposed mechanism of catechol extradiol dioxygenases (Solomon et al. 2000). Here we report the crystal structure of a eukaryotic 3HAO from Saccharomyces cerevisiae (Y3HAO) determined at 2.4 Å resolution. The Y3HAO structure and active site identified here are of critical importance to further understand the catalytic mechanism of 3HAO and the substrate specificity, and also to help in the design of 3HAO inhibitors to efficiently reduce the QUIN level and attenuate neurological deficits. On the other hand, as an extradiol dioxygenase, 3HAO may be utilized in degrading aromatic compounds.
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The asymmetric unit of the Y3HAO crystal contains two molecules related by noncrystallographic twofold symmetry axes (Fig. 2B). Residues 26–137 fold into two antiparallel -sheets 1
2
947 and 3856 (strands labeled in Fig. 2A), with nine strands forming a central -jelly roll barrel. The N-terminal residues 1–20 comprise an 1 helix and a short 310 helix at the C-terminal end, an additional -strand (0) at the N-terminal end that is antiparallel with the -sheet 74921 of the other dimer-related molecule and participates in the barrel formation. The jelly roll forms a cupin cavity corresponding to the catalytic site and containing a Ni2+ in the crystal structure. After the core -sheets are two additional anti- parallel -strands (1011), which form an extension to one face of the jelly roll. In a parallel arrangement with them, the longest helix (2) forms a lid over the active site. The loop between 10and 11 and the loop between 3 and C-terminal residues are linked with a coordinated Ni2+. This C-terminal segment is at the far end of the dimer (Fig. 2). The region acting as a lid over the active site appears to be very flexible, as evinced by the markedly high B factors comprising residues at loop 11–2 and N-terminal of 2, and functions as a gate controlling access to the active site. The dimer interface is formed principally by -sheet 012947 (Fig. 2), and the total area buried at the interface is 
2700 Å2 per subunit, corresponding to 30% of the subunit solvent-accessible surface area and resulting in the high degree of burial of hydrophobic residues (Trp12, Phe34, Val36, Trp56, Tyr58, Leu90, Ile108, Val110) at the interface.
The RMS distance between the 170 C atoms of subunit A and subunit B is 1.2 Å. The principal differences between the subunits occur in three surface loops, loop 1–1 (residues 21–25), loop 9–10 (residues 113–120), loop 11–2 (residues 138–144), and N-terminal of 2. These segments are flexible and consistent with their high temperature factors and may be involved in substrate entry and product release. In subunit B, loop 1– 1, 1, and 2 are closer than in subunit A. In the present Y3HAO structure, one of the bound nickel atoms occupies the proposed Fe2+-coordinated active site. It is coordinated by the N
1 atom of His49, two O atoms of Glu55, and the N2 atom of His97, with metal–ligand distances of 2.1–2.2 Å except for the Glu55 O1 atom where the distance is 2.5 Å, shorter than the distance of 2.7 Å from the Glu57 O1 to Fe3+ ion in the recently solved 3HAO from Ralstonia metallidurans (RM3HAO) (Zhang et al. 2005). The octahedral coordination environment is completed by two water molecules positioned further away from the metal center. In subunit A, the distance of the two water molecules to Ni2+ is 3.0 and 3.4 Å, respectively (Fig. 3). In subunit B of Y3HAO, the coordinate bond distances are similar to that of subunit A except that the coordinate bond distance of one of the water molecules to Ni2+ is 2.1 Å, and another water molecule to Ni2+ is 2.9 Å. In RM3HAO, the distance of the two water molecules to Fe3+ is the same and is 2.4 Å (Fig. 3). In solution, Y3HAO also appears as an intimate dimer identified by gel-filtration chromatography (data not shown). However, all of the mammalian 3HAOs characterized so far were found to be present and active as a monomer (33 kDa) (Calderone et al. 2002). Further sequence analysis suggests that the additional C-terminal segment present in metazoan enzymes may contribute to this dissimilarity (see below).
Structural comparison of Y3HAO and RM3HAO
The secondary structure and overall fold of the Y3HAO homodimer is very similar to that of RM3HAO. The crystal structure of RM3HAO reveals a monomer in the asymmetric unit; the monomers in adjacent asymmetric units interact, forming a dimer related by twofold symmetry. The sequence identity between Y3HAO and RM3HAO is 38%. Upon superposition of subunit A to that of RM3HAO, the RMS distance between the 169 C atoms is 1.5 Å. Figure 4 shows the superposition of the C backbones of the two structures, as well as structure-based sequence alignment of the corresponding sequences. 3HAO contains the two characteristic sequences of the cupin superfamily, namely G-(X)5-HXH-(X)3,4-E-(X)6-G and G-(X)5-PXG-(X)2-H-(X)3-N, each of which corresponds to two strands, separated by a less conserved region of 15–50 amino acids composed of another two strands with an intervening loop of variable length (Dunwell et al. 2001). In Y3HAO, these signature sequences are separated by 23 amino acids. The intervening loop, 5–6, has six residues (71–76), and three of them (Glu71, Asp73, and Glu75) are acidic . Glu71, with Arg123 and Tyr125 (two residues in 10), and Glu135 (in 11) form a hydrogen-bonding network and make the overall structure compact. Asp73, together with Asp70, Thr72, and Lys77, forms another hydrogen-bonding network, whereas the intervening loop in RM3HAO is shorter and has only two residues, Asp and Gly. In RM3HAO, Glu122 and Tyr124 (two residues in 10) and Arg134 and Glu136 (two residues in 11) form a hydrogen-bonding network with Arg94, a residue in loop 7–8. Another difference occurs in 1, which is two residues longer, and loop 1– 2 (residues 31–33), which is three residues shorter in Y3HAO. Differences occur also in loop 11–2, which is three residues longer than in RM3HAO, and 2 (residues 145–155), which is two residues shorter. These segments act as a lid region over the active site of RM3HAO and are more compact than that of Y3HAO.
The orientations and positions of the active-site residues —Asn43, Arg45, Asp47, His49, Glu55, Gln59, His97, Arg101, Glu111, Arg114, and Asp120—are especially well conserved, with only one conservative substitution at position 51, an Asn residue in yeast and an Asp residue in Ralstonia metallidurans (Fig. 4B), which suggests the same catalytic mechanism in prokaryotic and eukaryotic 3HAO. The km value of HAA of 19.2 µM for wild-type Y3HAO is similar to those obtained for RM3HAO (22.4 µM) and for the cloned H3HAO (2.3 µM) (Kucharczyk et al. 1998; Zhang et al. 2005). Loop 1–1 in RM3HAO is aligned well with subunit A of Y3HAO; furthermore, this loop in the complex structure of RM3HAO with substrate reveals a closed conformation, suggesting that substrate binding would induce a closed conformation. Buried hydrophobic residues (Phe34, Val36, Tyr58, Leu90) at the interface are conserved in the yeast enzyme (177 residues) and its prokaryotic homologs which are all of a similar length, indicative of a biological dimer, except that the O
atom of Ser88 of subunit A forms a bifurcated hydrogen bond with the N2 atom of His30 and the N1 atom of Trp56 of the other dimer-related subunit in yeast (Fig. 4A).
Alignment of 3HAO sequences
Using the program Clustal W (Thompson et al. 1994), we aligned the 30 most homologous 3HAO sequences and show six representative homologous 3HAO sequences (Fig. 4B). Based on the structure of Y3HAO, and the complex structures of RM3HAO with the inhibitor 4-chloro-3-hydroxyanthranilate (ClHAA) and either molecular oxygen or NO (nitric oxide), active site residues are strictly conserved among these 30 orthologous sequences. Iron-binding residues, including two histidine residues (His49 and His97) and a glutamic acid (Glu55), not only are conserved, but also are located in similar spatial arrangements (Fig. 5). Together with His49 and Glu55, four hydrophilic residues near the active iron site, Asp120 (or E), Asn51 (or D, E), Glu111, and Arg114 form a hydrogen-bonding network (Fig. 5); this hydrogen-bond network may participate in a charge-relay system and seems to be important in the catalysis of 3HAO. Two oxygen-binding residues, Arg45 and Asp47, help O2 bind to ferrous ion; upon the substrate binding, Arg45 moves toward the bound O2 molecule to form a hydrogen bond with the noncovalently bound oxygen atom, and at the same time Asp47 moves to Arg45 to keep two hydrogen bonds with Arg45 (Fig. 5) (Zhang et al. 2005). Residues Arg101, Gln59, and the substrate-binding hydrophobic pocket are also highly conserved; upon substrate binding, Arg101 forms two hydrogen bonds to the carboxylate group of the substrate, Gln59 forms a hydrogen bond with Arg101 (Zhang et al. 2005; Fig. 5), and the hydrophobic face of the substrate is located in a hydrophobic pocket, primarily formed by Phe57, Leu66 (or V), Tyr89 (or F), Pro99, and Val109. Asn43 may form a hydrogen-bond network with Arg45 and Arg101 by solvent molecules, and also presents in all homologs. Other conserved residues—Pro22, Pro23, Gly40, Gly62, and Pro92—are located at the loops, which are likely for maintaining structural integrity (Fig. 4B).
As has been predicted on the basis of primary sequence, the -jelly roll barrel subunit structure of 3HAO indicates that it is a member of a class of proteins known as cupins, with a double-stranded -helix fold in SCOP (Murzin et al. 1995) structural classification characterized by a conserved -barrel fold from which the name of the superfamily is derived. In spite of the low sequence identity among the superfamily (9%–20%), cupin is possibly the most functionally diverse protein superfamily described to date, comprising both enzymatic and nonenzymatic members, with either one or two cupin domains (Dunwell et al. 2004). With respect to the metazoan 3HAOs, the conservation of an extra C-terminal segment (100 residues) absent in the lower species is also obvious. Secondary structure of the C-terminal domain is predicted to be mainly eight -strands, much like the composition of the core N-terminal fold, and consistent with a circular dichroism analysis of the secondary structure of human 3HAO, which is mainly of strands and a minority of (Calderone et al. 2002). It tempted us to speculate that the C-terminal domain may also adopt a cupin fold to make the enzyme a bicupin monomer with a similar overall geometry as that of the Y3HAO dimer.
It is the first example of evolution from a monocupin dimer to bicupin monomer in the diverse cupin super-families. It is also a little reminiscent of the evolution of class I to class II of the type I extradiol dioxygenases (Spence et al. 1996), while the mutation and loss of function happened in the N-terminal domain to give class II. Alignments showed that these C-terminal domains of the metazoan 3HAOs share a low homology with their N-terminal portions as well as other known cupin sequences, reflecting a rather unconstrained evolution (Fig. 4B). The two conserved cupin sequence motifs are best conserved in the N-terminal domain, where the conserved histidine and glutamic acid residues correspond to the metal-coordinating residues. The C-terminal domain motifs lack the metal-binding residues normally associated with the cupin fold, which indicates an abolishment of metal binding and activity of the C-terminal domain. The C-terminal region is unrelated to the enzymatic reaction, against the proposed deprotonation function of His190 in human 3HAO (Mendel et al. 2004). Identification of the metazoan bicupin 3HAOs is of significance in that the higher species enzymes are experimentally intractable due to instability and inclusion body formation. An exception is human homo-gentisate dioxygenase (Titus et al. 2000), a hexamer arranged as a dimer of trimers, which also belongs to the type III non-heme ferrous extradiol dioxygenases; but it is an unusual type of cupin as it has the active site metal ion coordinated near the interface between subunits within the partially formed cupin domain, and it contains the metal binding site in its C-terminal domain. However, 3HAO shares a characteristic metal coordination site within the jellyroll in cupins as a monocupin dimer or bicupin monomer; therefore, 3HAO is a special subgroup of the type III extradiol dioxygenases.
Two other extradiol dioxygenases also cleave ortho–aminophenol: One of them is 2-aminophenol 1,6-dioxygenase (Lendenmann and Spain1996), which belongs to the type II extradiol dioxygenases; the other is 4-amino-3-hydroxybenzoate 2,3-dioxygenase (4A3HBA23D) from Bordetella sp. 10d (Murakami et al. 2004). 4A3HBA23D from Bordetella sp. 10d (175 residues), also as a biological dimer, has 30% and 24% identities with Y3HAO and 3HAO from Homo sapiens (H3HAO), respectively, and no identities with other extradiol dioxygenases. However, 3HAO and 4A3HBA23D show high substrate specificity only for their natural substrates, respectively, which differ in the position of an amino group. Figure 6 shows a sequence alignment of Y3HAO and 4A3HBA23D. Active-site residues Arg45, His49, Asn51, Glu55, His97, Glu111, Arg114, and Asp120 are identical; Asn43 and Asp47 are conservatively replaced by Glu46 and Glu50 in Bordetella sp. 10d. Two substrate-binding residues, Arg101 and Gln59, are replaced by Phe101 and Ser62, respectively, in Bordetella sp. 10d. The hydrophobic residues lining the substrate are highly conserved, except that Phe57 is replaced by hydrophilic residue Gln60 in Bordetella sp. 10d. Therefore, residues Arg101, Gln59, and Phe57 are crucial for the substrate specificity of 3HAO.
Metal coordination
The crystal structure of Y3HAO shows that the enzyme contains two nickel centers per monomer, in agreement with results from metal elementary analysis. One metal center is located at the end of the molecule and is solvent-exposed. The nickel ion is coordinated mainly by two typical Cys-XX-Cys motifs (Cys126, Cys129, Cys163 and Cys166) in the C-terminal sequence, with a tetrahedral geometry. This Cys-XX-Cys motif is common to the divalent metals. The nickel ion or the iron ion in the RM3HAO all may be introduced during purification, and the biologically relevant metal ion needs further study. There is strict conservation of this motif in the monocupin 3HAOs, but it is absent in the bicupin homologs. This metal center is apparently unrelated to enzymatic activity, and a structural stabilization role is proposed. Like RM3HAO, the two metal sites in Y3HAO are separated by 24 Å.
The experimental electron density map clearly reveals the presence of the other metal ion coordinated by the side chains of His49, Glu55, and His97 located in the -barrel. In fact, tertiary structure of the cupin domain has the advantage of providing a flexible "active site" within the center of the -barrel, resulting from the different metals bound by the relatively conserved ligands within the characteristic motifs in the superfamily. A ligand environment with three histidines (via their NE2 atoms) and one glutamate (via the OE2) has been observed in many cupin members such as germin with a Mn2+ center (Woo et al. 2000), phosphomannose isomerase with a Zn2+ center (Cleasby et al. 1996), oxalate decarboxylase with two Mn2+ centers (Anand et al. 2002), copper-or iron-containing quercetin 2,3-dioxygenase (Gopal et al. 2005), zinc ion-containing auxin-binding 1 protein (Woo et al. 2002), and a Ni2+-binding dioxygenase, acireductone dioxygenase (Pochapsky et al. 2002). In some members, just as in 3HAO, one of the three histidines is lost, resulting in a His2 Glu/Asp coordination sphere. This common 2-His-1-car-boxylate facial triad motif is also shared by many mononuclear non-heme iron(II) enzymes from different families that catalyze different reactions and have distinct requirements for catalysis. For example, 4-hydroxyphenylpyruvate dioxygenase (HPPD) (Fritze et al. 2004), one of the -ketoglutarate iron-dependent dioxygenases, and the predominant subclass of cupins, in spite of divergent structures, all feature an active site in which two histidines and one carboxylate ligand occupy one face of the iron(II) coordination sphere. This 2-His-1-carboxylate facial triad was proposed as a common platform to coordinate an iron(II) center in non-heme iron enzymes and is one of nature's recurring bioinorganic motifs (Koehntop et al. 2005). The three sites at the opposite face allow metal to bind O2 and a variety of substrates,providing the flexibility for the activesite to effect the remarkable range of reactions.
A comparison of the catalytic metal-binding site of 3HAO with the facial triads of known non-heme iron(II) oxygenase reveals an apparent difference: His49 in Y3HAO ligates the metal ion by the N1 atom rather than a N2 as in most of the oxygenases (Fig. 3), despite the similar overall geometry. The only exception is that in human homogentisate dioxygenase (HGO), a similar N1–Fe2+ ligation is observed on the spacial equivalent His335 (Titus et al. 2000). Both 3HAO and HGO catalyze aromatic ring-cleaving reactions different from the typical catechol extradiol dioxygenases, with one hydroxyl substituted by an ortho-amino or para-hydroxyl group, respectively. However, it was not mentioned by Titus et al. (2000), possibly due to an uncertainty that this kind of ligation would be preserved after substrate binding and during the reaction. In Y3HAO, a strictly conserved Asp120 on loop 9–10 limits the side chain of His49 by an O1–N2 hydrogen bond, and the electron density map clearly indicates the nearest atom in His49 to the metal ion should be at the position. Rotating the imidazole ring to form a similar N2–metal bond would need considerable movement of the main chain of 3 and disrupt the hydrogen bond to Asp120. Conformation of the active-site residues is sustained by the hydrogen-bonding network.
Active site and proposed catalytic mechanism
Despite the lack of overall structural similarity, the activesite structures of 3HAO and 2,3-dihydroxybiphenyl 1,2-dioxygenase (BphC) derived from Pseudomonas sp. strain KKS102 (Sato et al. 2002), one of the class II of the type I extradiol dioxygenases, are similar. Like BphC, the substrate HAA binds to the iron of RM3HAO as an asymmetrical bidentate ligand, at sites trans to the two imidazole ligands. Also, the oxygen atom adjacent to the C–C bond that is cleaved is ionized, in which C3-OH is deprotonated (Zhang et al. 2005). An initial deprotonation of the hydroxyl of the substrate is crucial for O2 activation; in RM3HAO, Glu110 forms a hydrogen bond with the C-3 hydroxyl group of HAA and deprotonates C3-OH. The O2 binding site is also opposite to the endogenous iron ligand Glu. These similarities suggest that there may have been a convergent evolution among extradiol dioxygenases and that they probably share similar catalytic mechanisms (Bugg and Lin 2001; Vaillancourt et al. 2002; Siegbahn and Haeffner 2004; Vetting et al. 2004; Viggiani et al. 2004).
On the basis of the coordinates of the RM3HAO–HAA complex structure, a HAA moiety was modeled into the active site of subunit A of Y3HAO, as seen in Figure 7. There is no major difference in the substrate binding pocket between Y3HAO and RM3HAO. The crystal structure of the RM3HAO–HAA complex shows clear differences from that of the native enzyme in that as loop 1–1, 1, loop 11–2, and 2 move toward the center of -barrel, the active site conformation is more closed, but the positions of the residues forming the hydrogen-bond network remain the same. Based on this, we propose a catalytic mechanism for 3HAO (Fig. 8). The first step of the reaction involves the displacement of one solvent ligand and O1 atom of Glu55 from the enzyme resting state (Fig. 8A) by the substrate to form a five-coordinate iron(II) species with a chelated monoanionic 3-hydroxyanthranilate (Fig. 8B); the substrate HAA binds to the iron as a bidentate ligand in which C3-OH is deprotonated. In the ES complex, the 3-hydroxy group of HAA forms a hydrogen bond to the O2 atom of Glu111; the hydrogen-bonding network makes it easy to induce deprotonation of C3-OH. Together with the hydrogen-bonding network, the O1 atom of Glu55 makes a hydrogen bond from the site opposite the C-2 amino group of the substrate HAA (Fig. 7). The carboxylate group of HAA forms two hydrogen bonds to Arg101, and the N2 atom of Gln59 forms a hydrogen bond with the NH1 group of Arg101; this interaction and hydrophobic interactions stabilize the substrate binding. The next step would then be O2 binding to the vacant site of the ES complex; its binding site is opposite to endogenous iron ligand Glu55. The O2 binding is supposed to induce complete deprotonation of the C2-NH2 group of the substrate (Fig. 8C). At this stage, the bound dioxygen molecule acquires a negative charge due to electron transfer from the metal center, resulting in the formation of an imine–Fe2+-superoxide intermediate. Because the bound dioxygen molecule is located in the cavity that is lined with a mixture of hydrophobic and hydrophilic residues, the negative charge on the superoxide may be stabilized by the NH2 group of Arg45 or the protonated Glu55 (Fig. 8C). Then the activated dioxygen molecule attacks the C3 atom of the substrate to give an iron–alkylperoxo intermediate (Fig. 8D), which undergoes alkenyl migration, Criegee rearrangement, and O–O bond cleavage to give an unsaturated seven-membered lactone intermediate and an iron(II)-bound hydroxide ion (Fig. 8E). The NH2 group of Arg45 or the protonated Glu55 assists cleavage of the O–O bond in the Criegee rearrangement, and iron(II)-bound hydroxide ion then hydrolyzes the lactone to afford product. The precise reaction mechanism will be solved by the complex structures of 3HAO–HAA with active site Fe2+ under anaerobic condition, and mutational studies.
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Structure determination
Data sets were collected at three wavelengths from a single selenomethionine derivative crystal at 100 K on Beamline F2 of MacCHESS, using energies corresponding to the peak (
1 = 0.9798 Å) and the edge (2 = 0.9802 Å) of the experimentally determined selenium K-edge. All processing, scaling, and merging of data sets were performed using the HKL2000 package (Otwinowski and Minor 1997). Initial phases were calculated to 3.5 Å resolution with SHARP (de la Fortelle et al. 1997) from seven heavy atom sites. DM (Cowtan 1999) was used for density modification and phase extension to 2.4 Å. A partial Y3HAO model was initially built using ARP/wARP (Perrakis et al. 1999), and then the sequence of Y3HAO was built into the resultant density maps using a threading model as a guide. The electron density allowed very clearly the identification of the two molecules in the asymmetric unit. Refinement was performed with Refmac5.0 (Murshudov et al. 1997) using the peak data, and the noncrystallographic symmetry constraints were released in the latter steps. The metal ions of Y3HAO (four per asymmetric unit) could be unambiguously detected in anomalous difference Fourier maps calculated from both the peak and the edge data. The Ni2+ was refined at full occupancy with a temperature factor of 36.7–42.8 Å2. The final model contains 348 residues, 60 water molecules, and 4 Ni2+ ions. The model was validated using PROCHECK (Laskowski et al. 1993). The Ramachandran plot produced by PROCHECK shows 91.2% of all the residues in the most favored regions, 8.1% in additional allowed regions, and 0.7% generously allowed regions. For details of the R-factor, Rfree, and stereochemistry of the final model, see Table 1.
Identification of the metal ion
The presence of the metals Mg, Ca, Fe, Co, Ni, and Zn were analyzed by an atomic absorption spectrophotometry experiment using PE 1100B, Atom abs (PE, USA). The results indicated that, after gel-filtration chromatography in 20 mM Tris-HCl (pH 8.5) and 150 mM NaCl, only Ni2+ (the molar ratio of Ni2+ to Y3HAO is 2.2) was concomitant with the protein, apparently introduced during the Ni2+-affinity chromatography step.
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Article published online ahead of print. Article and publication date are at http://www.proteinscience.org/cgi/doi/10.1110/ps.051967906.
Abbreviations: Y3HAO, 3-hydroxyanthranilic acid 3,4-dioxygenase from Saccharomyces cerevisiae; RM3HAO, 3-hydroxyanthranilic acid 3,4-dioxygenase from Ralstonia metallidurans; HAA, 3-hydroxyan-thranilate; QUIN, quinolinic acid; NMDA, N-methyl-D-aspartate; NAD+, nicotinamide adenine dinucleotide; AMPA, -amino-3- hydroxy-5-methyl-isoxazole; 4A3HBA23D, 4-amino-3-hydroxybenzo- ate 2,3-dioxygenase from Bordetella sp. 10d; HPPD, 4-hydroxyphenyl-pyruvate dioxygenase; HGO, human homogentisate dioxygenase; BphC, 2,3-dihydroxybiphenyl 1,2-dioxygenase from Pseudomonas sp. strain KKS102; MAD, multiple wavelength anomalous dispersion; EC, enzyme classification.
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Bugg T.D.H. and Lin G. 2001. Solving the riddle of the intradiol and extradiol catechol dioxygenases: How do enzymes control hydroperoxide rearrangements? Chem. Commun. 2001: 941–952.[CrossRef]
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clearly indicates an aspartate in this position. The map shown in green was superimposed on the refined 2.4 Å resolution coordinates of Y3HAO. Carbon (yellow), oxygen (red), and nitrogen (cyan) atoms are shown.
1) 310 helices. Fully conserved residues (white letters on black background) and conservatively substituted residues (black letters in black boxes) across this group of 3HAOs are indicated. (Black star) Residue in alternate conformations. The image was generated using the program ESPript (
