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First published online December 15, 2006; 10.1105/tpc.106.041376 The Plant Cell 18:3656-3669 (2006) © 2006 American Society of Plant Biologists OPEN ACCESS ARTICLE
Structural Basis for Dual Functionality of Isoflavonoid O-Methyltransferases in the Evolution of Plant Defense Responses[OA]
a Howard Hughes Medical Institute, Jack H. Skirball Center for Chemical Biology and Proteomics, Salk Institute for Biological Studies, La Jolla, California, 92037 2 To whom correspondence should be addressed. E-mail noel{at}salk.edu; fax 858-597-0855.
In leguminous plants such as pea (Pisum sativum), alfalfa (Medicago sativa), barrel medic (Medicago truncatula), and chickpea (Cicer arietinum), 4'-O-methylation of isoflavonoid natural products occurs early in the biosynthesis of defense chemicals known as phytoalexins. However, among these four species, only pea catalyzes 3-O-methylation that converts the pterocarpanoid isoflavonoid 6a-hydroxymaackiain to pisatin. In pea, pisatin is important for chemical resistance to the pathogenic fungus Nectria hematococca. While barrel medic does not biosynthesize 6a-hydroxymaackiain, when cell suspension cultures are fed 6a-hydroxymaackiain, they accumulate pisatin. In vitro, hydroxyisoflavanone 4'-O-methyltransferase (HI4'OMT) from barrel medic exhibits nearly identical steady state kinetic parameters for the 4'-O-methylation of the isoflavonoid intermediate 2,7,4'-trihydroxyisoflavanone and for the 3-O-methylation of the 6a-hydroxymaackiain isoflavonoid-derived pterocarpanoid intermediate found in pea. Protein x-ray crystal structures of HI4'OMT substrate complexes revealed identically bound conformations for the 2S,3R-stereoisomer of 2,7,4'-trihydroxyisoflavanone and the 6aR,11aR-stereoisomer of 6a-hydroxymaackiain. These results suggest how similar conformations intrinsic to seemingly distinct chemical substrates allowed leguminous plants to use homologous enzymes for two different biosynthetic reactions. The three-dimensional similarity of natural small molecules represents one explanation for how plants may rapidly recruit enzymes for new biosynthetic reactions in response to changing physiological and ecological pressures.
In sessile organisms such as plants, the need to rapidly evolve chemical defenses to changing environments is often met by the recruitment of enzymes into new metabolic pathways, resulting in the amazing diversity of plant secondary metabolism observed in nature (Pichersky and Gang, 2000  ). The isoflavonoid natural products of the Leguminosae act as antimicrobial phytoalexins during plant-fungal pathogen defense responses and as signaling molecules mediating bacterial or fungal symbioses (Dixon, 1999). Their biosynthesis diverges from the ubiquitous plant flavonoid pathway after the formation of committed flavanone intermediates, namely liquiritigenin or naringenin (Figure 1
). The oxidative aryl ring migration and coupled introduction of a 2-OH moiety catalyzed by the cytochrome P450 isoflavone synthase (IFS) (Hashim et al., 1990) together with the subsequent 4'-O-methylation of the IFS product, 2-hydroxyisoflavanone, comprise critical catalytic steps at the entry point into the formation of a structurally and functionally diverse group of isoflavonoid phytoalexins, including isoflavans, coumestans, and pterocarpans (Wong, 1975; Dewick, 1993; Dixon, 1999; Aoki et al., 2000).
Methylation of the C4' hydroxyl group of 2-hydroxyisoflavanone by a 4'-specific O-methyltransferase, HI4'OMT, recently identified in licorice (Glycyrrhiza echinata) (Akashi et al., 2003 ), yields 2-hydroxy-4'-O-methoxy-isoflavanone that undergoes dehydration to yield formononetin (7-hydroxy-4'-methoxyisoflavone) (Akashi et al., 2000; Aoki et al., 2000; Liu and Dixon, 2001; Akashi et al., 2005) (Figure 1). HI4'OMT is homologous to the previously characterized 6a-hydroxymaackiain 3-O-methyltransferase (HM3OMT) from pea (Pisum sativum; Preisig et al., 1989). Pea HM3OMT catalyzes the final O-methylation step in pea phytoalexin biosynthesis, converting the pterocarpan 6a-hydroxymaackiain into the antimicrobial end product pisatin (Preisig et al., 1989, 1991; Wu et al., 1997). This reaction is critical for resistance of pea against the fungal pathogen Nectria hematococca, virulent isolates of which possess a specific detoxifying cytochrome P450 enzyme, pisatin demethylase, located on a dispensable chromosome (VanEtten et al., 1980; Ciuffetti and VanEtten, 1996; Wasmann and VanEtten, 1996). Among several legumes, including pea, alfalfa (Medicago sativa), barrel medic (Medicago truncatula), and chickpea (Cicer arietinum), only pea species accumulate naturally the 3-O-methylated pterocarpanoid pisatin. However, feeding the pisatin precursor 6a-hydroxymaackiain to barrel medic suspension culture results in the formation of the 3-O-methylated pea product pisatin (see below). The high level of amino acid sequence similarity of barrel medic HI4'OMT with pea HM3OMT suggests that the two enzymes may possess dual activity for either 3- or 4'-O-methylation depending upon substrate availability. Therefore, HI4'OMTs represent fascinating examples of likely serendipitous functional redundancy in phylogenetically related plants that hold special significance for the evolution of defense responses in the Leguminosae. Here, we report the biochemical characterization of HI4'OMT from M. truncatula and the molecular basis of the dual functionality of HI4'OMT by determining the steady state kinetic parameters of HI4'OMT for each substrate and by elucidating the structures of HI4'OMT at high resolution with each substrate bound.
3-O-Methylation of Pterocarpans and Functional Identification of M. truncatula HI4'OMT/HM3OMT Like the forage legume alfalfa, M. truncatula (barrel medic) primarily accumulates the pterocarpanoid phytoalexin medicarpin (Figure 1). To test whether barrel medic also possesses the biosynthetic activity capable of 3-O-methylation of pterocarpans, such as 6a-hydroxymaackiain, leading to pisatin as found in pea, M. truncatula cell suspension cultures were fed 20 µM 6a-hydroxymaackiain for 36 h. Chromatographic analysis of phenolic extracts from the treated and control cells revealed the presence of a metabolite with the identical UV spectrum and retention time as an authentic pisatin standard (Figure 2 ). This feeding study provides analytical evidence that barrel medic cells contain an enzyme or enzymes capable of regiospecifically methylating a compound they do not make, namely 6a-hydroxymaackiain, resulting in the accumulation of a pea-specific phytoalexin, namely pisatin. In addition to detecting pisatin, an additional product identical in UV spectrum to the 6a-hydroxymaackiain substrate but differing in elution time was also detected in cell extracts. This compound is most likely the glycosylated conjugate of the fed 6a-hydroxymaackiain precursor, and experiments to ascertain this are under way.
To identify putative O-methyltransferases responsible for this unexpected activity, the pea HM3OMT sequence (GenBank accession number U69554) was used for BLAST searching of M. truncatula EST libraries. This bioinformatic analysis led to the identification of a full-length cDNA clone spanning 1.478 kb (Mt HI4'OMT; GenBank accession number AY942158), with 90% amino acid sequence identity to pea HM3OMT, 87% sequence identity to licorice HI4'OMT (accession number AB091684), and 51% sequence identity to alfalfa isoflavone 7-OMT (accession number U97125). Not unexpected given the high degree of sequence identity, phylogenetic analysis indicated that the HI4' OMTS from different legumes and the pea HM3OMT all clustered together and that this cluster was distinct from several other functionally characterized O-methyltransferases belonging to the same type I plant OMT family (Zubieta et al., 2001 ; Noel et al., 2003) (Figure 3
).
The protein encoded by the Mt HI4'OMT gene was expressed in Escherichia coli and purified with a hexa-His N-terminal tag. To obtain the hydroxyisoflavanone substrate that is not commercially available and is chemically unstable, 2,7,4'-trihydroxyisoflavanone was prepared biosynthetically using recombinant M. truncatula IFS incubated with a racemic mixture of 2R/2S-liquiritigenin (7,4'-dihydroxyflavanone) substrates (Figure 1). In this reaction, only the 2S-isomer served as an IFS substrate (data not shown), consistent with previous reports of IFS substrate specificity (Hagmann and Grisebach, 1984 ; Kochs and Grisebach, 1986). However, the 2,7,4'-trihydroxyisoflavanone product resulting from this IFS-catalyzed in vitro reaction existed as a pair of stereoisomers based upon rapid purification using chiral HPLC (data not shown). Given the instability of these hydroxyisoflavanone products, it was impossible to establish the stereochemistry of this mixture. This biosynthetically derived mixture of minimally two stereoisomers of 2,7,4'-trihydroxyisoflavanone was then used for kinetic analyses and also soaked into preexisting crystals of HI4'OMT complexed to the demethylated product of S-adenosyl-L-Met (SAM), S-adenosyl-L-homo-Cys (SAH) (see next section). Incubation of the recovered recombinant protein with 2,7,4'-trihydroxyisoflavanone obtained from the in vitro reaction of M. truncatula IFS with 7,4'-dihydroxyflavanone and the methyl donor SAM resulted in the accumulation of a methylated intermediate that was readily dehydrated to formononetin, indicative of 4'-OMT activity (Figures 4A to 4C ). Incubation of the recombinant protein with the pea compound 6a-hydroxymaackiain and SAM resulted in production of pisatin (Figures 4F and 4G). HI4'OMT was not active with di- or trihydroxylated isoflavones, including daidzein (Figure 4D) and genistein, or with the pterocarpans (–)-medicarpin and maackiain (data not shown).
The steady state kinetics of recombinantly expressed barrel medic HI4'OMT catalyzed methylation of 2,7,4'-trihydroxyisoflavanone and 6a-hydroxymaackiain were measured using various concentrations of substrates (the maximum concentration of 2,7,4'-trihydroxyisoflavanone or 6a-hydroxymaackiain achievable,  250 µM, was limited by their low solubility in the 100% methanol used for preparation of the stock solution and the final reaction buffer used for kinetic analysis) at a fixed concentration of SAM of 312.5 µM in the presence of AdoHcy nucleosidase to eliminate product inhibition by SAH (Hendricks et al., 2004). Methanol concentrations were held constant at 5% derived from the stock solution of substrate and additional methanol to compensate at low substrate concentrations. HI4'OMT exhibited an apparent Vmax= 35.9 ± 4.0 nmol·mg protein–1·min–1 and an apparent Km = 73.3 ± 20.2 µM for 2,7,4'-trihydroxyisoflavanone and an apparent Vmax= 17.9 ± 2.8 nmol·mg–1·min–1 and an apparent Km = 62.1 ± 25 µM for 6a-hydroxymaackiain. Apparent values were obtained because of the difficulties involved in obtaining saturating conditions for substrates. The kcat/Km (specificity constant) for 2,7,4'-trihydroxyisoflavanone is 334 ± 99.0 M–1·s–1, and for the pea compound, 6a-hydroxymaackiain, kcat/Km is 197 ± 85.0 M–1·s–1. Although the catalytic efficiency is slightly higher for 2,7,4'-trihydroxyisoflavanone (although arguably within experimental error of the measurements and calculations), HI4'OMT does exhibit nearly identical apparent affinity for both isoflavonoid compounds regardless of biological source. Finally, the steady state kinetic constants of HI4'OMT for the SAM cosubstrate (methyl donor) were measured at a fixed concentration of 2,7,4'-trihydroxyisoflavanone of 200 µM (near its solubility limit). HI4'OMT displays an apparent Vmax= 23.9 ± 3.0 nmol·mg–1·min–1 and apparent Km = 99.8 ± 32.4 µM. This latter value is within the range of previously reported estimates for isoflavonoid-specific OMTs (Wengenmayer et al., 1974; Preisig et al., 1989). While unlikely given the close correspondence of these values to previously reported values, it is possible that the apparent Vmax and Km could differ when using saturating concentrations of 6a-hydroxymaackiain.
Structural Determination by Protein X-Ray Crystallography
Previously, several crystal structures of phenylpropanoid and isoflavonoid-specific plant O-methyltransferases were determined with substrates and products bound. These catalytically and structurally similar enzymes were classified as plant type I OMTs (Noel et al., 2003 ), of which HI4'OMT and HM3OMT also belong. As originally noted in these previously published OMT crystal structures (Zubieta et al., 2001, 2002), HI4'OMT/HM3OMT also forms a well packed and substantially identical crystallographic dimer (Figure 5) that likely reflects the quaternary structure of the enzyme in solution and in cells. Each monomer consists of an N-terminal domain spanning 141 residues that primarily mediates dimerization but which partially constitutes the back wall of the active site cavity of the dyad-related neighboring polypeptide chain used for phenolic substrate recognition. A large C-terminal domain spanning 223 residues forms the core SAM/SAH binding module (Rossmann fold) that is shared with the type I, type II, and type III families of plant SAM-dependent small molecule methyltransferases (Noel et al., 2003) (Figure 5).
Structural Comparisons of HI4'OMT/HM3OMT with Other Plant Type I OMTs
SAH/SAM Cosubstrate Binding Pockets In the HI4'OMT/HM3OMT structures presented here, helix  14, ß-strands ß3, ß4, and ß6 and the connecting loops form a cleft where the demethylated product SAH resides (Figure 7
). One wall of the SAH/SAM binding cleft is lined by the side chains of Asp-250, Met-251, Phe-252, Leu-263, Trp-265, Val-266, and Trp-270 and Ile-278, while the opposing wall is lined by the side chains of Val-206, Val-213, Phe-229, Val-234, and the apolar portions of Asp-230 and Gln-231 (data not shown). Together, both walls of the SAH/SAM binding site form a greasy crevice facilitating van der Waals interactions with SAH/SAM. The carboxyl moiety of Asp-230 forms hydrogen bonds with the 2' and 3' Rib hydroxyl groups of SAH, while the carboxyl group of Asp-250, the side chain amino moiety of Lys-264, and the peptide bond carbonyl oxygen of Gly-207 form a hydrogen bond network with the exocyclic amino group of the adenine ring and the free carboxyl and amino moieties of SAH, respectively. Finally, the carboxyl group of Asp-205 tethers the amino group and carboxyl moieties of SAH through water-mediated hydrogen bonds (Figure 7).
Stereoselective Binding Mode of HI4'OMT for Phenolic Substrates In contrast with the previous prediction of 2R,3S configurations at C2 and C3 of the IFS product 2,7,4'-trihydroxyisoflavanone (Hashim et al., 1990 ; Sawada et al., 2002; Akashi et al., 2003), x-ray crystallographic analysis revealed that 2,7,4'-trihydroxyisoflavanone obtained from in vitro IFS reactions, HPLC purified under nonchiral resolving conditions, and then soaked into HI4'OMT crystals possesses the 2S,3R stereochemical configuration (Figure 8A
). Moreover, in the HI4'OMT structures solved with either pea 6a-hydroxymaackiain or pea pisatin bound, the conformations of the 6aR,11aR-stereoisomers of these pea compounds observed in the phenolic binding pocket of the barrel medic HI4'OMT (Figure 8B) are identical to the conformation of 2S,3R-2,7,4'-trihydroxyisoflavanone described above. So while the pea compounds are chemically distinct from 2,7,4'-trihydroxyisoflavanone, all of the compounds share a nearly identical three-dimensional shape when bound to HI4'OMT that is complementary to the shape of its active site cavity, thus explaining the dual functionality of this enzyme in solution.
The 2S,3R configuration of 2,7,4'-trihydroxyisoflavanone bound in the catalytic cavity resides in a conformation in which the planes formed by the A and C rings, respectively, sit nearly perpendicular to the plane of the B ring linking the A and C rings. This apparently stably bound conformation of the HI4'OMT 2-hydroxyisoflavanone product fits snuggly in the Y-shaped phenolic substrate binding cavity, resulting in the proper positioning of the 4'-hydroxyl group on the B ring for transmethylation (Figure 8C). The specific binding of 2S,3R-2,7,4'-trihydroxyisoflavanone is predominantly achieved through a complementary binding pocket formed by a contiguous van der Waals surface in a Y-shaped active site. This cavity consists of hydrophobic side chains, a large fraction of which are aromatic and Met residues. In particular, Met-179 and Met-322 form a thioether clamp that constrains the orientation of the B ring, while Met-325 and Met-374 form a second more widely spaced clamp for restraining the A and C rings. Most noticeable, the 2-hydroxyl group of 2S,3R-2,7,4'-trihydroxyisoflavanone serves as a key link for anchoring the bound molecule in the active site cavity (Figure 8C).
For the HI4'OMT structures solved with either 6a-hydroxymaackiain or pisatin bound, the plane formed by rings A and B of the pterocarpans orient nearly orthogonal to the C, D, and E rings, generating a sharply bent conformation that occupies the same Y-shaped binding cleft previously noted for 2S,3R-2,7,4'-trihydroxyisoflavanone. Moreover, the 6a-hydroxyl moiety of the pterocarpans acts much like the 2-hydroxyl group of 2,7,4'-trihydroxyisoflavanone in anchoring and orientating the methyl acceptor through a direct hydrogen bond with the hydroxyl moiety of Tyr-25 from the dyad-related polypeptide chain (Figure 8D). Negligible activity is observed when maackiain, the biosynthetic precursor of (6aR,11aR)-6a-hydroxymaackiain, bearing a similar stereoconfiguration but lacking the 6a-hydroxyl moiety, is employed in barrel medic HI4'OMT or pea HM3OMT assays (Preisig et al., 1989
The large conformational differences of the N-terminal domains relative to the C-terminal SAM/SAH binding domains among previously solved plant type I OMTs and HI4'OMT results in a large cleft between the SAM/SAH binding surfaces and the phenolic substrate binding pockets. This cleft leaves a large solvent-exposed active site in HI4'OMT relative to the more compact arrangement of each domain observed previously in I7OMT (Zubieta et al., 2001 ). This open architecture of HI4'OMT results in a 7- to 10-Å distance between the methyl donor SAM, the catalytic base His-268, and the methyl accepting hydroxyl moiety of phenolic substrates bound against the wall formed by the N-terminal domain. Another plant type I OMT, namely, caffeic acid/5-hydroxyferulic acid 3/5-O-methyltransferase (COMT) whose crystal structure was previously determined in our laboratory, possesses a similar open architecture (Zubieta et al., 2002).
Together, these current and past OMT crystal structures implicate a functionally important conformational change associated with phenolic substrate recognition, binding, catalysis, and product release in plant type I OMTs. Given the large accessible surface area buried in the plant type I OMT dimer (
Based upon the crystal structures presented here, the 2S,3R-stereoisomer of 2,7,4'-trihydroxyisoflavanone is specifically recognized by HI4'OMT/HM3OMT (Figure 9
). IFS, which is used to prepare 2,7,4'-trihydroxyisoflavanone, was previously shown to accept only 2S-flavanones as substrates (Hagmann and Grisebach, 1984
The demonstration of the 3R aryl group configuration bound to HI4'OMT/HM3OMT implicates a potentially facile skeletal rearrangement of the IFS product before HI4'OMT/HM3OMT-directed recognition and methylation. This observation implies that the putative 2R,3S stereoisomer of 2,7,4'-trihydroxyisoflavanone formed by IFS undergoes reversible transformation that ultimately leads to the formation of four diastereomeric structures in solution, each of which differs with respect to their ground state stability and conformation.
Finally, the close structural similarity of the 6a-hydroxylated 6aR,11aR-pterocarpan, 6a-hydroxymaackiain, with 2S,3R-2,7,4'-trihydroxyisoflavanone accounts for the observed dual activities of HI4'OMT toward two seemingly distinct isoflavonoid-derived substrates. Therefore, our biochemical and structural studies explain the recognition and stereospecific turnover of chemically distinct small molecules by highly similar plant type I OMTs. As such, this form of metabolic serendipity represents an example of possible short cuts to rapid evolutionary adaptation in organisms possessing a biosynthetically rich chemical repertoire for ecological interactions. The concept of substrate promiscuity in enzymes has been suggested to offer evolutionary advantages in organisms as they adapt to new environments and evolve new enzyme activities (O'Brien and Herschlag, 1999
The observation that barrel medic contains an enzyme with efficient in vitro catalytic activity for a compound (6a-hydroxy-6aR,11aR-pterocarpan) that it does not make is explained by the nearly identical three-dimensional structures for the 2S,3R-stereoisomer of 2,7,4'-trihydroxyisoflavanone and for the 6aR,11aR-stereoisomer of 6a-hydroxymaackiain bound to HI4'OMT. Given how similar the overall conformations of these two substrates are, it is difficult to imagine how limited mutational changes in HI4'OMT could lead to variants specific for only one of the substrates in question since changes are likely to affect activity against either substrate. Moreover, since both activities are necessary in pea for pisatin biosynthesis, it is possible that the related enzyme from pea, HM3OMT, carries out both methylations. Indeed, silencing of the Ps HM3OMT gene by antisense or sense constructs in pea hairy root cultures not only greatly reduced the accumulation of pisatin but also resulted in undetectable amounts of 6a-hydroxymaackianin. The lack of 6a-hydroxymaackianin accumulation was most likely due to silencing of the earlier 4'-O-methylation biosynthetic step possibly exploiting the dual activity of HI4'OMT/HM3OMT described here (Wu and VanEtten, 2004
Materials and Chemicals Pisatin and maackiain were generous gifts from Hans VanEtten (University of Arizona). (–)-Medicarpin and 6a-hydroxymaackiain were from our lab collection (R.A.D.). All other flavonoids and isoflavonoids used in the study were purchased from Indofine. SeMet, thrombin, SAM, and S-adenosyl-L-homo-Cys (SAH) were purchased from Sigma-Aldrich. Radiolabeled adenosyl-L-Met-S-(methyl-14C) was purchased from PerkinElmer Life Sciences. The pET28a(+) expression vector and Escherichia coli strain BL21(DE3) were purchased from Novagen. Ni2+-NTA resin was purchased from Qiagen. Benzamidine Sepharose and Superdex 200 FPLC columns were obtained from Amersham Bioscience.
Feeding of 6a-Hydroxymaackiain to Medicago truncatula Suspension Cultures and Metabolite Analysis
Isolation and Identification of M. truncatula cDNAs Encoding HI4'OMT/HM3OMT
Phylogenetic Analysis of Barrel Medic HI4'OMT
Biosynthesis and Purification of 2,7,4'-Trihydroxyisoflavanone
Expression was performed according to the EasySelect Pichia expression kit manual. Yeast cells were collected and resuspended in 0.1 M potassium phosphate, pH 8.0, containing 0.4 M Suc, 14 mM ß-mercaptoethanol, and 1x protease inhibitors (Complete EDTA-free Protease Inhibitor Cocktail tablets; Roche Diagnostics). Microsomes were isolated as described (Liu et al., 2003
Activity Assays of Barrel Medic HI4'OMT
For MS analysis, an HP 1100 series II LC system (Hewlett-Packard) with a photodiode array detector was coupled to a Bruker Esquire ion-trap mass spectrometer (MSD trap XCT system) equipped with an electrospray ionization source. A reverse phase, C18, 5-µm, 4.6 x 250-mm column (Phenomenex) was used. The mobile phase consisted of 0.2% (v/v) formic acid (positive-ion mass spectra) or 0.1% (v/v) acetic acid (negative-ion mass spectra) using Gradient II as described above. The flow rate to the MSD trap was 0.5 mL/min (positive-ion spectra) or 0.8 mL/min (negative-ion spectra), and the temperature of the column was kept at 25°C. The positive-ion mass spectra were acquired for the enzymatic reactions with 2,7,4'-trihydroxyisoflavanone substrate, and negative-ion mass spectra were acquired for the enzymatic reactions with 6a-hydroxymaackiain. Positive-ion electrospray ionization was performed using an ion source voltage of 3.5 kV and a capillary offset voltage of 158.6 V. Nebulization was aided with a coaxial nitrogen sheath gas provided at a pressure of 50 p.s.i. Desolvation was aided using a counter current nitrogen flow set at a pressure of 11 p.s.i. and a capillary temperature of 350°C. Mass spectra were recorded over the range 50 to 1000 m/z. Negative-ion electrospray ionization was performed using an ion source voltage of 3.0 kV and a capillary offset voltage of 70.7 V. Nebulization and desolvation were aided as described above. Mass spectra were recorded over the range 50 to 2200 m/z. The ion trap mass spectrometer was operated under an ion current control of
Rates of HI4'OMT-mediated methylation of the substrates 6a-hydroxymaackiain and 2,7,4'-trihydroxyisoflavanone were determined using various concentrations of each substrate (1.25, 2.5, 5, 10, 20, 40, 80, 100, 150, 200, and 250 µM) with the total SAM concentration fixed at 312.5 µM and augmented with 0.0042 µCi of adenosyl-L-Met-S-(methyl-14C). The reactions were performed in a total volume of 60 µL of Tris-HCl buffer, pH 8.0, as described above at 30°C for 15 min. Ten micrograms of purified HI4'OMT and 1.5 µg of recombinant AdoHcy nucleosidase were simultaneously added to the reaction mixture to initiate transmethylation. The nucleosidase irreversibly cleaves SAH to adenine and S-ribosylhomocysteine, thus reducing SAH-mediated product inhibition of HI4'OMT (Hendricks et al., 2004
Protein X-Ray Crystallography
Crystals of HI4'OMT in complex with SAH and pisatin were obtained by cocrystallization of protein with 2.5 mM of SAH and
During refinements, structure factors obtained from intensity data were used to generate SIGMAA-weighted 2Fo – Fc and Fo – Fc electron density maps with phases calculated from the structure of the current model. Inspection of the electron density maps and model building were performed in O (Jones et al., 1991 For the HI4'OMT-SAH-2,7,4'-trihydroxyisoflavanone complex, 90.3, 7.8, and 1.9% of the residues were found in the most favored, the allowed, and the generously allowed regions of the Ramachandran plot, respectively, with a G factor of 0.35. No residues were found in the disallowed region. For the HI4'OMT-SAH-(6a)-hydroxymaackiain complex, 93.5, 5.6, and 0.9% of the residues were found in the most favored, the allowed, and the generously allowed regions of the Ramachandran plot, respectively, with a G factor of 0.34. For the HI4'OMT-SAH-pisatin complex, 91.8, 7.3, and 0.9% of the residues were found in the most favored, the allowed, and the generously allowed regions of the Ramachandran plot, respectively, with a G factor of 0.26. No residues were found in the disallowed region.
Coordinates and Accession Numbers
We thank Michael B. Austin for valuable discussion on data processing, Daneel Ferreira for helpful discussions concerning IFS stereochemistry, and Hans VanEtten for the generous gift of maackiain and pisatin. This work was supported by the National Science Foundation under Grant 0236027 to J.P.N. C.-J.L. was supported in part by a senior postdoctoral fellowship from the Noble Foundation. The work done in the Brookhaven National Laboratory was supported by the Laboratory Directed Research and Development program to C.-J.L. under contract with the Department of Energy. B.E.D. was supported by a grant from the Oklahoma Center for the Advancement of Science and Technology to R.A.D. Portions of this research were carried out at SSRL, a national user facility operated by Stanford University on behalf of the U.S. Department of Energy, Office of Basic Energy Sciences. The SSRL Structural Molecular Biology Program is supported by the Department of Energy, Office of Biological and Environmental Research, and by the National Institutes of Health, National Center for Research Resources, Biomedical Technology Program. J.P.N. is an investigator of the Howard Hughes Medical Institute.
1 Current address: Department of Biology, Colorado State University, Fort Collins, CO, 80525.  The author responsible for distribution of materials integral to the findings presented in this article in accordance with the policy described in the Instructions for Authors (www.plantcell.org) is: Joseph P. Noel (noel{at}salk.edu).
[OA] Open Access articles can be viewed online without a subscription. www.plantcell.org/cgi/doi/10.1105/tpc.106.041376 Received January 23, 2006; Revision received October 26, 2006. accepted November 5, 2006.
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ABSTRACT
INTRODUCTION
. While the axial positions of the hydroxy-phenyl and hydroxyl moieties clearly represent higher-energy conformations, HI4'OMT presumably uses binding energy to selectively sequester the 2,7,4'-trihydroxyisoflavanone substrate.
