2.1. Chemicals

Benzoyl-CoA, malonyl-CoA, naringenin and 4-hydroxy­coumarin were all purchased from Sigma (USA); 4-coumaroyl-CoA was purchased from TransMIT (Germany). 3,5-Dihydroxybi­phenyl was prepared as described previously by Nilsson & Norin (1963) and was purified with a Waters preparative LCMS FractionLynx system using mass and UV-directed fractionation on an XBridge Prep OBD C18 5 µm 30 × 100 mm column, with a gradient from 5:95:0.1(v:v:v) water:acetonitrile:formic acid to acetonitrile (0.1% formic acid) over 8 min with a flow rate of 30 ml min⁻¹. Its identity was confirmed by comparison of its ¹H NMR spectrum in MeOD-d₄ and m/z values with those reported in the literature (Liu et al., 2004). Salicoyl-CoA (2-hydroxybenzoyl-CoA) was prepared as described elsewhere (Sidenius et al., 2004) and was purified via preparative LCMS as described above. The identity of salicoyl-CoA was confirmed by comparison of its ¹H NMR spectrum in MeOD-d₄ and m/z values with those reported in the literature (Guo et al., 2009).

2.2. Cloning and recombinant protein expression and purification

cDNAs for MdCHS2, MdBIS1 and MdBIS3 were derived from a cDNA library of M. domestica and inserted into the pBluescript SK+ vector in the laboratory of A. C. Allan and R. P. Hellens at The New Zealand Institute for Plant and Food Research Ltd (Newcomb et al., 2006). For recombinant expression, the MdCHS2, MdBIS1 and MdBIS3 cDNAs were inserted between the NcoI and EcoRI restriction sites of the expression vector pHIS8 which, under the control of a T7 promoter, yields target proteins fused to an N-terminal octahistidine tag (Jez, Ferrer et al., 2000). Subcloning occurred as follows. Firstly, NcoI digestion sites were added to each pBluescript template using the QuikChange (Agilent) PCR method following the manufacturer's protocol. The primers used were MdCHS2-forward, 5′-CTCGACGGTCACCATGGTTTTTATATCCGATCGTCGAGAAAGATC-3′; MdCHS2-reverse, 5′-GATCTTTCTCGACGATCGGATATAAAAACCATGGTGACCGTCGAG-3′; MdBIS1-forward, 5′-TAACCAAAGGCGCCATGGGGCAAGTTGAAGAGC-3′; MdBIS1-reverse, 5′-GCTCTTCAACTTGCCCCATGGCGCCTTTGGTTA-3′; MdBIS3-forward, 5′-CTCATTCTTAACCAAAGGCGCCATGGAGCTAGTTAAAGAGCAGATATAAA-3′; MdBIS3-reverse, 5′-TTTATATCTGCTCTTTAACTAGCTCCATGGCGCCTTTGGTTAAGAATGAG-3′ (NcoI sites are underlined and the translation start sites are shown in bold). Plasmid preparations (Qiagen) of NcoI-mutated pBluescript constructs were digested with NcoI and EcoRI. The approximately 1.2 kb digestion fragments were gel-purified and ligated with NcoI/EcoRI-digested pHIS8. The correct reading frames for the pHIS8 constructs were obtained using the QuikChange PCR method and the following sets of primers: MdCHS2-forward, 5′-TCCGCGTGGTTCCATGGTGACCGTCG-3′; MdCHS2-reverse, 5′-CGACGGTCACCATGGAACCACGCGGA-3′; MdBIS1 and MdBIS3-forward, 5′-TCCGCGTGGTTCCATGGCGCCTTTGG-3′; MdBIS1 and MdBIS3-reverse, 5′-CCAAAGGCGCCATGGAACCACGCGGA-3′ (NcoI sites are underlined and the translation start sites are shown in bold). All primers were purchased from Integrated DNA Technologies. The fidelity of all constructs was confirmed by sequencing (Eton Biosciences, USA).

Expression constructs were heterologously overexpressed in E. coli BL21 (DE3) (Novagen) expression hosts. E. coli cultures were grown at 37°C in TB medium (Invitrogen) to an optical density (600 nm) of 1.0, induced with 0.5 mM isopropyl β-D-thiogalactopyranoside and allowed to grow overnight at 22°C. Bacterial cells were harvested by centrifugation, resuspended in lysis buffer [50 mM Tris–HCl pH 8.0, 500 mM NaCl, 20 mM imidazole, 1%(v/v) Tween 20, 10%(v/v) glycerol, 10 mM β-mercaptoethanol] and lysed by sonication. Recombinant proteins were isolated from the E. coli lysate by affinity chromatography with nickel–nitrilotriacetic acid-coupled agarose (Qiagen) and eluted with buffer (lysis buffer without detergent) containing 250 mM imidazole. During the first dialysis (50 mM Tris–HCl pH 8.0, 500 mM NaCl, 10 mM β-mercaptoethanol), the recombinant proteins were treated with thrombin for cleavage of the octahistidine tag. The final purification step consisted of gel filtration of the protein extracts on a Superdex 200 FPLC column equilibrated with 50 mM Tris pH 8.0, 500 mM NaCl, 10 mM β-mercaptoethanol. Protein fractions were pooled, dialyzed into 12.5 mM Tris pH 8.0, 125 mM NaCl, 5 mM DTT, concentrated to at least 10 mg ml⁻¹ and finally stored at −80°C. SDS–PAGE analysis was used to confirm the protein purity. Protein concentrations were determined using the absorbance at 280 nm.

A codon-optimized synthetic gene for benzophenone synthase from Hypericum androsaemum (HaBPS), GenBank accession AAL79808, as reported by Liu et al. (2003) was purchased from GenScript (Piscataway, New Jersey, USA). The initial HaBPS construct (pUC57 vector) was digested with NcoI and BamHI, gel-purified and ligated with NcoI/BamHI-digested pHIS8. The correct reading frame of the HaBPS pHIS8 construct was achieved using QuikChange PCR and the primers HaBPS-forward, 5′-CTGGTTCCGCGTGGTTCCATGGCCAATTC-3′, and HaBPS-reverse, 5′-GAATTGGCCATGGAACCACGCGGAACCAG-3′ (NcoI sites are underlined and the translation start sites are shown in bold). Primers were purchased from Integrated DNA Technologies (USA) and the sequence of the final pHIS8 construct was confirmed by sequencing (Eton Biosciences, USA).

2.3. qPCR analysis of MdCHS2, MdBIS1 and MdBIS3 gene expression

Tissues from M. domestica `Royal Gala' were collected and qPCR analyses of gene expression were performed as described previously (Henry-Kirk et al., 2012; Dare et al., 2013). In brief, all reactions were performed using the LightCycler 480 SYBR Green I Master Mix (Roche Diagnostics) according to the procedure described by the manufacturer. qPCR reactions were performed four times using 5 µl SYBR Green Master Mix, 0.5 µl forward primer, 0.5 µl reverse primer, 1 µl water and 3 µl cDNA template (Table 1). A negative water control was included in each run. Fluorescence was measured at the end of each annealing step. Amplification was followed by a melting-curve analysis with continual fluorescence data acquisition during the 65–95°C melt. Actin from M. domestica (GenBank accession CN938023) was selected as the reference gene because of its consistent transcription level throughout fruit tissues and leaves. The results were interpreted using the LightCycler480 software platform.

2.4. Crystallization of MdCHS2, MdBIS3 and HaBPS

Crystals of MdCHS2, MdBIS3 and HaBPS were grown by the hanging-drop vapor-diffusion method using buffered protein solutions (10–15 mg ml⁻¹) mixed with equal volumes of the reservoir solution and incubated at 4°C. Typical reservoir solutions were 14% PEG 8000, 0.3 M ammonium acetate, 0.1 M sodium MOPSO pH 7.0 for MdCHS2 and 14% PEG 8000, 0.3 M ammonium acetate, 0.1 M sodium HEPES pH 7.5 for MdBIS3. Crystals of HaBPS grew from reservoirs consisting of 18%(w/v) PEG 8000, 0.1 M PIPES buffer pH 6.5. Crystal-soaking experiments were conducted by transferring apo MdBIS3 crystals into fresh drops containing reservoir plus 15 mM benzoyl-CoA and incubating overnight at 4°C. MdCHS2 and MdBIS3 crystals grew within 48 h, while HaBPS crystals typically grew within one week.

2.5. X-ray diffraction data collection

Crystals were transferred to a cryoprotectant solution consisting of reservoir solution supplemented with 20%(v/v) racemic 1,3-butanediol, prior to immersion in liquid nitrogen. X-ray diffraction data were measured from cooled crystals using ADSC Quantum 315 CCD detectors on beamlines 8.2.1 and 8.2.2 of the Advanced Light Source, Lawrence Berkeley National Laboratory. Diffraction intensities were indexed and integrated with MOSFLM (Leslie, 2006) and SCALA (Evans, 2006) in the CCP4 software suite (Collaborative Computational Project, Number 4, 1994; Potterton et al., 2003; Winn et al., 2011).

2.6. X-ray structure determination of MdCHS2, MdBIS3 and HaBPS

Initial crystallographic phases for apo crystals were determined by molecular replacement with Phaser (McCoy et al., 2007). Homology models of MdCHS2 and MdBIS3 were constructed with MODELLER (Šali & Blundell, 1993) based on the structure of chalcone synthase from Medicago sativa (PDB entry 1bi5; Ferrer et al., 1999). A homology model of HaBPS was generated using the crystallographic model of MdBIS3 as a template. These homology models served as the starting models for molecular replacement. The PHENIX suite of programs (Adams et al., 2010) was used to rebuild these initial structural models and for subsequent structural refinements. Coot (Emsley & Cowtan, 2004) was used for graphical map inspection and manual rebuilding of atomic models. Programs from the CCP4 suite were employed for all other crystallographic calculations. Molecular visualizations were generated with PyMOL (Schrödinger).

2.7. In vitro enzyme assays

Steady-state kinetic analyses were performed for chalcone synthase (EC 2.3.1.74), benzophenone synthase (EC 2.3.1.220) and biphenyl synthase (EC 2.3.1.177 and EC 2.3.1.208) activities. Standard enzyme assays for MdCHS2 consisted of 0.1 M potassium phosphate buffer pH 7.0, 0.5 µM protein, 60 µM coumaroyl-CoA and 100 µM malonyl-CoA in a total volume of 500 µl. Standard enzyme assays for MdBIS1 and MdBIS3 consisted of 0.1 M potassium phosphate buffer pH 7.0, 0.1 µM protein, 15 µM starter substrate, 60 µM malonyl-CoA in a total volume of 500 µl. Assays for HaBPS consisted of 0.1 M potassium phosphate buffer pH 7.0, 0.1 µM protein, 20 µM starter substrate and 80 µM malonyl-CoA in a total volume of 500 µl. The reactions were initiated by the addition of protein and were quenched with acetic acid [5%(v/v)] after 10 min incubations at 37°C, except for MdCHS2, which was incubated for 5 min at 37°C. Kinetic constants were determined using six substrate concentrations with the concentration of the second substrate held constant. Product formation for each protein was linear with respect to incubation time and protein concentration. After quenching, samples were extracted with ethyl acetate, dried under vacuum and then resuspended in 40 µl methanol. Each substrate–enzyme series was assayed in triplicate, and kinetic constants were calculated using a product standard curve and nonlinear regression analyses in GraphPad Prism (GraphPad Software).

Product formation was analyzed by LC-MS with an Agilent 1100 series LC-MSD instrument containing a Gemini (4.6 × 150 mm, 5 µm particle size) reversed-phase column. Chromatographic separations employed a flow rate of 0.5 ml min⁻¹ and a linear gradient with the initial and final mobile phases consisting of 95%(v/v) water, 5%(v/v) acetonitrile, 0.1%(v/v) formic acid and 5%(v/v) water, 95%(v/v) acetonitrile, 0.1%(v/v) formic acid, respectively. The detection wavelengths were 228 nm (3,5-dihydroxybiphenyl), 288 nm (4-hydroxy­coumarin and naringenin) and 306 nm (phlorobenzo­phenone). Products were confirmed by mass determination and reference to the chromatographic elution of authentic standards.

2.8. Molecular phylogenetics

Amino-acid sequences were aligned using the PROMALS3D web server (Pei et al., 2008) and phylogenetic analysis used the Jones–Taylor–Thornton substitution model (Jones et al., 1992) within the MEGA7 software package (Kumar et al., 2016).

2.9. Data deposition

The cDNA sequences have been deposited in GenBank with accession numbers JQ582624 for MdCHS2, JQ582625 for MdBIS1 and JQ582626 for MdBIS3. Crystallographic models have been deposited in the PDB with the accession codes listed in Table 2.

3.1. Functional characterization of CHS, BIS and BPS

Initially, we isolated three cDNAs from an apple cDNA library (M. domestica `Royal Gala') that showed similarity to plant type III PKSs. BLAST searches and analysis of the apple genome showed that one of the cDNAs was >96% identical in amino-acid sequence to chalcone synthases from Malus (Dare et al., 2013). The other two cDNAs were 92–99% identical in amino-acid sequence to biphenyl synthases from Sorbus aucuparia and M. domestica `Holsteiner Cox' (Liu et al., 2007, 2010; Chizzali et al., 2011). Based on sequence similarities, functional studies and phylogenetic analyses (see below), we named the above genes identified in this study MdCHS2, MdBIS1.1 and MdBIS3.1. For the sake of brevity, MdBIS1.1 and MdBIS3.1 will be referred to as MdBIS1 and MdBIS3 in this manuscript.

In vitro assays confirmed the biochemical activity of MdCHS2 as a chalcone synthase and of MdBIS1 and MdBIS3 as biphenyl synthases (Table 2). MdCHS2 was active with 4-coumaroyl-CoA; however, neither biphenyl or benzo­phenone products (see below) could be detected when benzoyl-CoA was used as the starter substrate. Both MdBIS1 and MdBIS3 were active with benzoyl-CoA and salicoyl-CoA, producing 3,5-dihydroxybiphenyl and 4-hydroxycoumarin, respectively. We did not detect significant differences between MdBIS1 and MdBIS3 in their catalytic efficiencies for benzoyl-CoA compared with salicoyl-CoA. In contrast to the observations by Chizzali et al. (2011) that the MdBIS1 homolog in `Holsteiner Cox' occurred as a nonfunctional allele, our biochemical analyses showed that MdBIS1 from `Royal Gala' is a functional enzyme.

To verify that the cloned MdCHS2, MdBIS1 and MdBIS3 genes were expressed, we analysed their gene-expression profiles in apple tissues (Fig. 2). Transcripts of MdBIS1 were unexpectedly observed to be most abundant in the root tips and main roots of apples and were nearly absent in all other tissues. The MdBIS1 transcript accumulation in root tips was approximately equal to the accumulation of MdCHS2 transcripts in apple fruit skin 128 d after full bloom. CHS significantly contributes to the pigmentation of apple fruit skin, which reaches a maximum at approximately 128 d after full bloom in Royal Gala (Henry-Kirk et al., 2012). Transcript accumulation of MdBIS3 was similar to MdCHS2 in apple fruit skin 100 d after full bloom.

Figure 2 qPCR analysis of MdCHS2, MdBIS1 and MdBIS3 gene-expression patterns in various tissues of M. domestica `Royal Gala'. dafb, days after full bloom.

For comparative purposes, we obtained a synthetic gene derived from the gene sequence of H. androsaemum BPS (HaBPS). Similar to previous reports, HaBPS produced 2,4,6-trihydroxybenzophenone (phlorobenzophenone) when incubated with benzoyl-CoA (Table 2; Liu et al., 2003). Biphenyl products were not detected. Additionally, unlike MdBIS1 and MdBIS3, 4-hydroxycoumarin was not detected when HaBPS was incubated with salicoyl-CoA as a starter substrate.

3.2. Overall structures of MdCHS2, MdBIS3 and HaBPS crystals

The crystal structures of MdCHS2, HaBPS and MdBIS3 were solved by molecular replacement (Table 3). All crystals contained the physiologically relevant twofold rotationally symmetric homodimer in their asymmetric unit (Fig. 3). The crystallographic model of MdCHS2 contained 774 out of 778 residues. The crystallographic models of HaBPS and MdBIS3 contained 772 out of 790 residues and 757 out of 776 residues, respectively. Lastly, the crystallo­graphic model of MdBIS3 complexed with benzoyl-CoA contained 756 out of 780 residues. The missing residues of all crystallo­graphic models were at the N- and C-termini of each monomeric subunit. Additionally, each monomer of MdBIS3 contained electron density consistent with 1,3-butanediol, the cryoprotectant. When superposed, the polypeptide backbones of MdCHS2 and MdBIS3 have an r.m.s.d. of 0.9 Å, those of MdCHS2 and HaBPS have an r.m.s.d. of 0.7 Å and those of MdBIS3 and HaBPS have an r.m.s.d. of 0.9 Å. Our final crystallographic models of MdCHS2 and HaBPS were refined at 2.1 Å resolution (R = 16.6%; R_free = 20.9%) and 2.85 Å (R = 20.1%; R_free = 26.1%), respectively. The final crystallographic models of apo MdBIS3 and MdBIS3 complexed with benzoyl-CoA were refined at 1.17 Å (R = 10.6%; R_free = 12.6%) and 1.20 Å (R = 11.1%; R_free = 13.1%), respectively, the highest resolution structures obtained to date for a type III PKS.

Figure 3 Overall crystal structures of MdCHS2, MdBIS3 and HaBPS. (a) The asymmetric units of MdCHS2 (blue), MdBIS3 (green) and HaBPS (brown) contain the physiologically relevant homodimers. The polypeptide chains of each protein are represented as ribbons. The side chains of the active-site cysteines for each crystal structure are shown as sticks and labeled with asterisks. The N-terminus and C-terminus of the superposed structures are labeled N and C, respectively. The dashed box highlights the CoA tunnel and the displaced solvent loops near the CoA tunnels of BIS and BPS (see Fig. 4). (b) The structure of BIS complexed with benzoyl-CoA. The surface of the protein dimer is displayed and each monomeric subunit is shown in ribbon representation with rainbow coloring from the N-terminus (blue) to the C-terminus (red). Benzoyl-CoA is displayed as spheres with atoms color-coded according to element: carbon, black; oxygen, red; phosphorus, orange; nitrogen, blue; sulfur, yellow.

Crystallographic analysis of secondary-structural elements between MdCHS2, HaBPS and MdBIS3 revealed only minor differences in topology, none of which immediately explained the differences in substrate specificity and terminal cyclization preferences during catalysis. The five-layered αβαβα topology of secondary-structural elements of each monomer is consistent with the `thiolase fold' originally observed in thiolase and present in all known structures of type III PKSs (Austin & Noel, 2003; Mathieu et al., 1994). Each monomer of MdCHS2, MdBIS3 and HaBPS contains two cis-peptide bonds at the dimer interfaces which are well defined by the electron densities of each structure and are conserved in all known type III PKSs. Structural differences between the superposed C^α traces of MdCHS2, HaBPS and MdBIS3 occur primarily at the solvent interface. In particular, a three-residue solvent-exposed loop in MdBIS3 and HaBPS is displaced approximately 5 Å toward the CoA tunnel compared with MdCHS2 (Fig. 3a).

3.2.1. CoA tunnel

A conserved arrangement of hydrogen bonds assists in the binding of CoA substrates in the CoA tunnels of MdBIS3, HaBPS and MdCHS2. Despite the use of reducing agents in all buffers and crystallization solutions, the electron-density maps indicated that the active-site cysteines of the MdBIS3 crystals were oxidized to their sulfinic acid derivatives (–SO₂H). Oxidation of active-site cysteines has been observed in other type III PKS structures (PDB entries 1bi5 and 1qlv) and prevents the transfer of substrates onto the active-site cysteines (Jez, Austin et al., 2000; Ferrer et al., 1999). Nonetheless, insight into substrate binding was provided by co-crystallization of MdBIS3 with benzoyl-CoA, resulting in intact benzoyl-CoA molecules with partial occupancies in both monomers of MdBIS3 (Figs. 3b and 4a). In MdBIS3, the side chains of residues Lys50 and Arg53 as well as the backbones of Ala305 and Gly302 form hydrogen bonds to the phosphates and pantetheine subunits of benzoyl-CoA, respectively. These hydrogen bonds are conserved in other type III PKS structures containing bound CoA substrates (PDB entries 1bq6 and 1ee0; Ferrer et al., 1999; Jez, Austin et al., 2000). However, as mentioned above, both MdBIS3 and HaBPS contain a three-residue solvent-exposed loop that is displaced significantly toward the CoA tunnel (Fig. 4b). The displaced loop in the MdBIS3–benzoyl-CoA complex generates an additional hydrogen bond between the adenine unit of benzoyl-CoA and the backbone carbonyl of Leu262. The displaced loops found in MdBIS3 and HaBPS appear to correlate with the rotameric state of one of the gatekeeper residues (Fig. 4c). The gatekeeper residues, Phe215 and Phe265 in MdCHS2, separate the CoA tunnel from the internal active-site cavity and affect substrate selectivity by acting as a steric gate during substrate binding (Ferrer et al., 1999; Jez et al., 2002). Phe265 of CHS is replaced with tyrosine in both MdBIS3 (Tyr260) and HaBPS (Tyr269). Differences in the side-chain torsion angles of Tyr260 in MdBIS3 (χ₁ = 61°) and Tyr269 in HaBPS (χ₁ = 50°) compared with Phe265 of CHS (χ₁ = 170°) significantly reorient the tyrosine side chains and increase the conformational flexibility of the nearby Leu262 in MdBIS3 and Leu271 in HaBPS. Lastly, the side-chain conformation of Tyr260 in MdBIS3 is stabilized via the presence of a water-mediated hydrogen bond to the backbone carbonyl of Phe192. The F265Y mutation in CHS was one of three mutations needed to shift the substrate specificity of CHS towards benzoyl-CoA (Liu et al., 2003). Presumably, a similar water-mediated hydrogen bond stabilizes Tyr269 of HaBPS; however, the lower resolution of the diffraction data for the HaBPS crystals prevented the analysis of waters.

Figure 4 Binding interactions of benzoyl-CoA. (a) Co-crystallization of MdBIS3 with benzoyl-CoA. MdBIS3 is displayed as a green cartoon; benzoyl-CoA is displayed in ball-and-stick representation. Hydrogen bonds are shown as dashed lines and waters are shown as spheres. Atoms are color-coded according to element: carbon, black; oxygen, red; nitrogen, blue; sulfur, yellow. The 2Fo − Fc OMIT electron-density difference map surrounding the benzoyl-CoA ligand is displayed as blue-colored cages and contoured at σ = 1.0 with carve = 1.3. (b) Overlay of the MdBIS3–benzoyl-CoA complex with MdCHS2 and HaBPS. Residues associated with the displaced solvent-exposed loop near the CoA tunnel and mutations near the benzoyl moiety of benzoyl-CoA are displayed as sticks. (c) Overlay of the MdBIS3–benzoyl-CoA complex with MdCHS2 and HaBPS rotated approximately 120° counterclockwise from that shown in (b).

3.3. Active-site architectures of CHS, BIS and BPS

3.3.1. Substrate loading

The active-site cavity of MdCHS2 is conserved and isomorphous with the previously characterized cavity of M. sativa CHS (Ferrer et al., 1999). In contrast, the active-site cavities of MdBIS3 and HaBPS contain a series of hydrophobic residues that block access to the 4-coumaroyl-CoA binding region of CHS. Residues of the MdCHS2 pocket include Ser133, Glu192, Thr194, Thr197, Gly216 and Ser338. Ser133, Glu192 and Thr914 are conserved in MdBIS3 as Ser128, Glu187 and Thr189, while Thr197, Gly216 and Ser338 are replaced with Phe192, Ala211 and Gly335. The conspicuous replacement of Thr197 in MdCHS2 with Phe192 in MdBIS3 reshapes the bottom of the MdBIS3 cavity (Fig. 5a). Furthermore, Phe192 sterically clashes with the carbonyl of naringenin derived from coumaroyl-CoA when the previously characterized CHS–naringenin complex is superposed onto MdBIS3 (Fig. 5b; Ferrer et al., 1999). Although Thr197 of MdCHS2 is conserved in HaBPS (Thr200), the electron density of Thr200 in HaBPS supports a rotamer with the methyl group of threonine protruding up into the coumaroyl-binding pocket of CHS (Fig. 5a). A significant change in the HaBPS cavity arises from the small-to-large replacement of Leu263 in MdCHS2 with Met267 in HaBPS. The side chain of Met267 in HaBPS is in the same vicinity of the active-site cavity as the Phe192 side chain of BIS, and similarly clashes with the carbonyl unit of naringenin derived from coumaroyl-CoA in the CHS–naringenin complex (Fig. 5b). Met267 of HaBPS is replaced with Phe258 in MdBIS3. The orientation of the side chain of Phe258 away from the binding pocket suggest that it is not directly involved in binding benzoyl-CoA, although it may assist in stabilizing the conformation of Phe192 in MdBIS3. Lastly, Gly256 is on the surface of the MdCHS2 cavity near the CoA tunnel; in MdBIS3 and HaBPS this position contains the slightly bulkier Ala. Mutations that increase the bulkiness of the side chain of position 256, including G256A, have previously been shown to shift the substrate specificity of CHS towards smaller substrates (Jez, Austin et al., 2000). Collectively, hydrophobic mutations in the active sites of MdBIS3 and HaBPS provide hydrophobic surfaces for interacting with small hydrophobic substrates such as benzoyl-CoA.

Figure 5 Active-site architectures of MdCHS2, MdBIS3 and HaBPS. (a) The internal cavities of MdCHS2 (blue), MdBIS3 (green) and HaBPS (brown) are displayed as surface representations. Residues lining the cavities are displayed; the catalytic triads of each protein are labeled with black asterisks. Red asterisks highlight residues in CHS that are known to affect benzoyl-CoA substrate specificity. The novel pockets of MdBIS3 and HaBPS are labeled with magenta arrows. Residues are colored according to element: oxygen, red; nitrogen, blue; sulfur, yellow. (b) Naringenin, the product of CHS activity with 4-coumaroyl-CoA as a substrate, is modeled into the cavities of MdCHS2, HaBPS and MdBIS3. Naringenin is displayed in ball-and-stick representation. Coordinates for naringenin were obtained from superpositioning of the CHS–naringenin complex (PDB entry 1cgk). C atoms of the naringenin ligand are colored black and all other elements are colored as described above.

3.3.2. Elongation and cyclization within benzoic acid-specific type III PKSs

The replacement of Ser338 in MdCHS2 with Gly generates a novel pocket in the active-site cavities of MdBIS3 and HaBPS associated with their elongation and cyclization reactions. Ser338 of MdCHS2 resides at the intersection of the coumaroyl-binding pocket and elongation/cyclization cavity and stabilizes the conformation of elongated polyketide intermediates (Jez, Austin et al., 2000). The replace­ment of Ser338 in CHS with Gly in both MdBIS3 (Gly335) and HaBPS (Gly342) allows the internal cavities of MdBIS3 and HaBPS to expand behind their respective active-site cysteines to generate novel pockets (Fig. 5a). The sides of this novel pocket in MdBIS3 are formed from the side chains of Cys125, Ala127, Ala157, Glu187 and Ala336 as well as the main-chain atoms of Gly158, Ala157, Gly335 and Ala336. Similarly, the side chains of Thr135 and Glu195 and the main-chain atoms of Gly166, Gly342 and Ser343 line the sides of this novel pocket in HaBPS. Notably, Klundt et al. (2009) observed that mutagenesis of Thr135 in HaBPS disrupted chain elongation and cyclization specificity.

The structural determinants of cyclization specificity in benzoic acid-specific type III PKSs are distinct from the previously described `aldol switch' of STSs. As mentioned above, CHS and BPS catalyze terminal Claisen cyclizations of their polyketide intermediates, while STS and BIS catalyze terminal aldol cyclizations (Fig. 1). Previously, the emergence of a subtle water-mediated hydrogen-bond network involving the side chains of Thr132, Glu192 and Ser338 (CHS numbering) was found to underlie aldol-cyclization reactions in STSs (Austin, Bowman et al., 2004; Shomura et al., 2005; Fig. 6a). The aldol switch of STSs is disrupted in BIS by the replacement of Thr132 and Ser338 of MdCHS2 with Ala (Ala127) and Gly (Gly335), respectively (Fig. 6b). Both Ala127 and Gly335 line the sides of the novel pocket formed in the active-site cavity of MdBIS3. While there are ordered waters present in the novel pocket of MdBIS3 which could function similarly to the nucleophilic water of the STS aldol switch, the lower resolution diffraction data of HaBPS prohibited further structural comparisons.

Figure 6 Structural elements contributing to cyclization specificity in MdCHS2, MdBIS3 and HaBPS. (a) The aldol-switch residues of stilbene synthase (PDB entry 1u0u) superposed onto MdCHS2 (blue). Residues are displayed as sticks. Atoms are color-coded according to element: oxygen, red; nitrogen, blue; sulfur, yellow. Water is shown as a cyan sphere. Hydrogen bonds are shown as dashed lines with associated distances in Å. (b) Active-site regions of MdBIS3 and HaBPS, homologous to the stilbene aldol switch, are overlayed and displayed as sticks.