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ORIGINAL RESEARCH article

Front. Plant Sci., 30 March 2016
Sec. Plant Physiology
This article is part of the Research Topic Molecular Mechanisms Underlying Polyamines Functions in Plants View all 15 articles

Structural Investigations of N-carbamoylputrescine Amidohydrolase from Medicago truncatula: Insights into the Ultimate Step of Putrescine Biosynthesis in Plants

\r\nBartosz SekulaBartosz Sekula1Milosz Ruszkowski*Milosz Ruszkowski2*Maura Malinska,Maura Malinska2,3Zbigniew DauterZbigniew Dauter2
  • 1Institute of Technical Biochemistry, Faculty of Biotechnology and Food Sciences, Lodz University of Technology, Lodz, Poland
  • 2Synchrotron Radiation Research Section, Macromolecular Crystallography Laboratory, National Cancer Institute, Argonne, IL, USA
  • 3Faculty of Chemistry, University of Warsaw, Warsaw, Poland

Putrescine, 1,4-diaminobutane, is an intermediate in the biosynthesis of more complexed polyamines, spermidine and spermine. Unlike other eukaryotes, plants have evolved a multistep pathway for putrescine biosynthesis that utilizes arginine. In the final reaction, N-carbamoylputrescine is hydrolyzed to putrescine by N-carbamoylputrescine amidohydrolase (CPA, EC 3.5.1.53). During the hydrolysis, consecutive nucleophilic attacks on the substrate by Cys158 and water lead to formation of putrescine and two by-products, ammonia and carbon dioxide. CPA from the model legume plant, Medicago truncatula (MtCPA), was investigated in this work. Four crystal structures were determined: the wild-type MtCPA in complex with the reaction intermediate, N-(dihydroxymethyl)putrescine as well as with cadaverine, which is a longer analog of putrescine; and also structures of MtCPA-C158S mutant unliganded and with putrescine. MtCPA assembles into octamers, which resemble an incomplete left-handed helical twist. The active site of MtCPA is funnel-like shaped, and its entrance is walled with a contribution of the neighboring protein subunits. Deep inside the catalytic cavity, Glu48, Lys121, and Cys158 form the catalytic triad. In this studies, we have highlighted the key residues, highly conserved among the plant kingdom, responsible for the activity and selectivity of MtCPA toward N-carbamoylputrescine. Moreover, since, according to previous reports, a close MtCPA relative from Arabidopsis thaliana, along with several other nitrilase-like proteins, are subjected to allosteric regulation by substrates, we have used the structural information to indicate a putative secondary binding site. Based on the docking experiment, we postulate that this site is adjacent to the entrance to the catalytic pocket.

Introduction

Polyamines (PAs) are small, aliphatic, polycationic compounds that bear at least two amino groups. Although PAs are found in all domains of life, the most abundant PA in nature is 1,4-diaminobutane, commonly named putrescine (PUT), which, together with 1,5-diaminopentane, cadaverine (CAD), owes its name to the noxious odor of putrefying cadavers. More complexed PAs include, but are not restricted to, triamine spermidine (SPD), tetraamine spermine (SPM) and thermospermine. It has been shown that PAs are some of the key players during plant growth and development, as well as response to both abiotic and biotic stresses (Do et al., 2014; Jimenez-Bremont et al., 2014; Minocha et al., 2014; Tiburcio et al., 2014; Liu et al., 2015). To list only a few examples, exogenous application of PUT can enhance thermotolerance of wheat (Kumar et al., 2014) and alleviate salt stress in apple callus (Liu et al., 2006). Also, supplementation with SPD mitigated salt stress symptoms in tomato and sorghum (Zhang et al., 2015; Yin et al., 2016). Application of exogenous PAs was shown to be not the only way to improve stress tolerance by increasing PA levels. Overexpression of genes involved in PA biosynthesis results in accumulation of PAs and, therefore, greater stress tolerance (Roy and Wu, 2001; Capell et al., 2004; Kasukabe et al., 2004; Alcazar et al., 2010; Wang et al., 2011). PAs are also related to nodulation, i.e., the symbiotic interaction between a plant hosts from legume (Fabaceae) family and nitrogen-fixing bacteria. Medicago truncatula (Mt), which is the source organism of the enzyme studied in this work, is a model legume plant. Legumes form special organs, root nodules, which are dwelled by nitrogen-fixing bacteria from Rhizobium genus. This extraordinary plant–microbe symbiosis allows legume plants to overcome limited nitrogen availability because rhizobia utilize atmospheric N2 and convert it into ammonia, which plants are able to assimilate. It has been demonstrated that the concentration of PAs affects both number and biomass of root nodules (Vassileva and Ignatov, 1999; Terakado et al., 2006). Moreover, PA levels in the nodule tissue are elevated by a factor of 5–10, when compared to the rest of the plant organs (Fujihara et al., 1994; Efrose et al., 2008).

For years, the molecular function of PAs was attributed only to their cationic character, that is, affinity to interact with negatively charged biomolecules, such as nucleic acids and proteins, and modulate transcription and translation (Bachrach, 2010; Gill and Tuteja, 2010; Igarashi and Kashiwagi, 2010; Tiburcio et al., 2014). Meanwhile, PAs can also regulate membrane transport (Pottosin and Shabala, 2014; Pottosin et al., 2014a) or stimulate antioxidant systems and quenching of reactive oxygen species (Shi et al., 2010; Xu et al., 2011; Radhakrishnan and Lee, 2013; Shu et al., 2013; Kamiab et al., 2014; Mostofa et al., 2014; Pottosin et al., 2014b).

In plant cells, the homeostasis of PAs is attained by regulation of their biosynthesis, catabolism, conjugation and transport (Liu et al., 2015). The elementary PA that plants biosynthesize is PUT. Synthesis of SPD and SPM involves enzymatic conjunction of PUT with aminopropyl groups from decarboxylated S-adenosylmethionine. There are two routes leading to PUT synthesis (Figure 1) (Martin-Tanguy, 2001). One originates from ornithine, which, in a single reaction, catalyzed by ornithine decarboxylase (ODC, EC 4.1.1.17), is converted into PUT. In the other pathway, arginine is the starting molecule, and some plants, such as Arabidopsis thanliana (At), rely solely on this method (Hanfrey et al., 2001). The arginine route involves three enzymatic steps: (i) arginine decarboxylation to agmatine by arginine decarboxylase (ADC, EC 4.1.1.19); (ii) deimination of agmatine by agmatine iminohydrolase (AIH, EC 3.5.3.12) and (iii) hydrolysis of N-carbamoylputrescine (NCP) to putrescine by N-carbamoylputrescine amidohydrolase (CPA, EC 3.5.1.53), with the release of carbon dioxide and ammonia. The latter enzyme, CPA from Medicago truncatula (MtCPA), is the subject of the studies presented here.

FIGURE 1
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FIGURE 1. Two pathways for putrescine biosynthesis. The reaction catalyzed by MtCPA is highlighted in blue.

Plants are the only eukaryotes able to produce PUT from arginine, which makes enzymes involved in PUT biosynthesis good targets for herbicide design. It has been shown that the plant pathway originates from bacteria (Illingworth et al., 2003; Fuell et al., 2010). Even though all three enzymes, ADC, AIH and CPA are examples of endosymbiotic horizontal gene transfer, they are encoded by nuclear DNA. It is, however, not surprising, as for instance a big part of cyanobacterial genes has been incorporated into the A. thaliana genome (Martin et al., 2002). Only ADC contains chloroplast-targeting signal peptide, whereas AIH and CPA are present in cytoplasm (Illingworth et al., 2003). Consistently, only the ADC sequence is present in many cyanobacteria, meanwhile most cyanobacteria use single agmatine ureohydrolase (EC 3.5.3.11) instead of AIH and CPA (Fuell et al., 2010).

N-carbamoylputrescine amidohydrolase enzymes belong to nitrilases, and more precisely, to C-N hydrolases breaking non-peptide bonds using Cys-Glu-Lys catalytic triad (Bork and Koonin, 1994; Pace and Brenner, 2001; Chen et al., 2003). Enzymatic activity of A. thaliana CPA (AtCPA) has been examined by Piotrowski et al. (2003). Using protein overexpressed in Escherichia coli cells, authors reported that AtCPA does not follow Michaelis–Menten kinetics, and its enzymatic activity can be described by Hill equation. The reported Hill coefficient, equal 2.2, indicated positive cooperative binding. The maximal velocity, Vmax was calculated as 86 nanokatals per mg of protein, and half maximal velocity was achieved at 135 μM of NCP. Based on native gel electrophoresis, authors also show that AtCPA in solution forms homooctamers (Piotrowski et al., 2003).

Even though the overall mechanism catalyzed by nitrilase enzymes has been established, particular subclasses must have evolved several modifications that allow for binding chemically different substrates. So far, there have been no structural information on any CPA enzyme from whichever domain of life. Therefore, it has been unknown how CPAs catalyze the enzymatic reaction, and which amino acid residues interact with the substrate and/or product. It also has been elusive what is the mechanism of the positive cooperative binging. In this studies, we address those fundamental questions, and using the first crystal structures of a CPA protein, expand the knowledge about these housekeeping enzymes.

Materials and Methods

Cloning, Overexpression and Purification of MtCPA

MtCPA protein was produced using a protocol adapted from the reported previously for obtaining δ1-pyrroline-5-carboxylate reductase from the same organism, (Ruszkowski et al., 2015). M. truncatula leaves were used for isolation of the total RNA with RNeasy Plant Mini Kit (Qiagen). cDNA was obtained with the use of SuperScript II reverse transcriptase (Life Technologies) and oligo dT (15 and 18) primers. PCR with the primers (Forward: TACTTCCAATCCAATGCCATGGCGGAAGACAAGGGTAGAAAAGTA and Reverse: TTATCCACTTCCAATGTTATCACAGAACAGGATTTTTGCCGTCCAAA) and cDNA as a template was performed to obtain the coding sequence of MtCPA open reading frame. The PCR product was incorporated into pMCSG68 vector (Midwest Center for Structural Genomics) by ligase-independent cloning (Kim et al., 2011). The N-terminus of the expressed protein contains His6-tag, followed by the TEV protease cleavage site, and non-cleavable Ser-Asn-Ala linker that precedes the genuine sequence of MtCPA.

BL21 Gold E. coli competent cells (Agilent Technologies), transformed with the vector, were used for overexpression of the protein. Culture was carried out to the A600 of 1.0 at 37°C in LB media with the addition of ampicillin (150 μg/ml). The culture was cooled to 18°C before induction. Then, IPTG (final concentration of 0.5 mM) was added to the culture. The culture was grown for 20 h and then cooled to 4°C. Cells were pelleted by centrifugation at 3500 × g for 20 min. After the supernatant removal, cells were resuspended in 35 ml of the binding buffer (50 mM Tris-HCl pH 8.0; 500 mM NaCl; 20 mM imidazole; 1 mM TCEP) and frozen at -80°C. Thawed culture was subjected to sonication to disrupt the cells. Bursts of total 4 min duration, with appropriate intervals for cooling, were applied. Disrupted cells were pelleted by centrifugation at 25 000 × g for 30 min at 4°C. The supernatant was used to retrieve the His6-tagged MtCPA protein on the column packed with 5 ml of HisTrap HP resin (GE Healthcare), which was connected to the Vacuum Manifold (Promega). After application of the supernatant, column was washed five times with 40 ml of the binding buffer. The elution of MtCPA was performed with 20 ml of elution buffer (50 mM Tris-HCl pH 8.0; 500 mM NaCl; 300 mM imidazole; 1 mM TCEP). His6-tagged TEV protease was added to the sample to the final concentration of 0.1 mg/ml to cleave the His6-tag. The sample was dialyzed overnight at 4°C against the buffer: 50 mM Tris-HCl pH 8.0; 500 mM NaCl; 1 mM TCEP. HisTrap HP resin was used to remove the cleaved His6-tag and the His6-tagged TEV protease. Final purification was performed by the size exclusion chromatography on HiLoad Superdex 200 16/60 column (GE Healthcare), equilibrated with the buffer: 50 mM Tris-HCl pH 8.0, 200 mM NaCl and 1 mM TCEP. The column was connected to the AKTA FPLC system (Amersham Biosciences).

MtCPA-C158S mutant was obtained by introduction of the C158S mutation to the vector used for overexpression of wild-type MtCPA, according to the Polymerase Incomplete Primer Extension method (Klock and Lesley, 2009). Primers used for PCR reaction were designed as follows – Forward: GCTATTTCCTGGGATCAGTGGTTTCCGGA and Reverse: ATCCCAGGAAATAGCGACTCCAATTTTCGCATA. The same protocol of overexpression and purification as for MtCPA was used in case of MtCPA-C158S. Sequences of MtCPA and MtCPA-C158S mutant were confirmed by DNA sequencing.

Crystallization and Data Collection

Both, MtCPA and MtCPA-C158S mutant proteins, were concentrated with Amicon concentrators (Millipore) to 20 mg/ml, as determined by the absorbance measurement at 280 nm, with the extinction coefficient of 38640. Initial crystallization trials were performed by sitting drop vapor diffusion method using the crystallization robot (Mosquito). Conditions were established for MtCPA as the 64th reagent of PEG/Ion Screen HT (Hampton research). Both proteins were then crystallized manually by hanging drop method in the conditions containing 20% PEG3350 and 8% Tacsimate at pH 7.0 (Hampton Research) or 20% PEG3350, 8% Tacsimate at pH 7.0 and 10% glycerol (GOL). Crystals with the best morphology were obtained by streak seeding.

Complexes of MtCPA with N-(dihydroxymethyl)putrescine (DHMP) and MtCPA-C158S with PUT were obtained by incubation of the unliganded proteins with PUT (10 mM final concentration) for 15 min. Samples were then centrifuged at 17 000 × g before crystallization setup. The complex of MtCPA with CAD was formed using the same protocol, with the final 17 mM concentration of CAD. Crystals were cryoprotected by transfer to the solution containing 20% PEG3350, 8% Tacsimate at pH 7.0 and 25% GOL, supplemented with the appropriate ligand.

The diffraction data were collected at Southeast Regional Collaborative Access Team (SER-CAT) 22-ID beamline at the Advanced Photon Source, Argonne National Laboratory, USA. The diffraction images were processed with XDS (Kabsch, 2010); for details see Table 1.

TABLE 1
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TABLE 1. Data-collection and refinement statistics.

Structure Determination and Refinement

Initial data of MtCPA were processed to the resolution of 2.65 Å. The online version of BALBES, a molecular-replacement pipeline (Long et al., 2008) was used for structure determination. Twenty-one structures with at least 15% identity to the given MtCPA sequence were recruited by BALBES. Subsequently, six structures with the best similarity of 39.6% along a 96-residue fragment were used for the structure determination. The following models from the PDB (Berman et al., 2000) were used: 3IVZ, 2W1V, 1F89, 1ERZ, 2VHH and 3AA0. All possible space groups in the orthorhombic system were tested. The best solution was obtained using the model 1ERZ with 574 residues in two monomers. Eight dimers of 1ERZ were found in the asymmetric unit of the MtCPA crystal lattice. The given model and the quality of electron density maps were inspected in Coot (Emsley et al., 2010). PHENIX AutoBuild (Terwilliger et al., 2008) was used for the model building, starting from the solution obtained from BALBES. After rebuilding, the model was taken for the successive steps of manual and automatic refinement with Coot and REFMAC5 (Murshudov et al., 2011). This model was used for the determination of all isomorphous MtCPA and MtCPA-C158S complexes by rigid body refinement. The refinement procedures were following: ligands and solvent molecules were deleted; the atomic displacement parameters were reset to 20 Å2 for all atoms and rigid body refinement was used in the first refinement cycle. At the later stages of the structure refinement, TLS parameters (Winn et al., 2001, 2003) were introduced. Restraints for DHMP were generated using PHENIX eLBOW (Moriarty et al., 2009) based on the chemical formula, while all the other ligands were refined against standard CCP4 libraries (Winn et al., 2011). The quality of refined structures was controlled by Rwork, Rfree factors (Brunger, 1992) and geometric parameters. PROCHECK (Laskowski et al., 1993) and MolProbity (Chen et al., 2010) were used for evaluation of the final models. Summary of data collection and refinement statistics are given in Table 1.

Docking

Docking calculations were carried out using Autodock version 4.2.6 (Morris et al., 2009). Non-polar hydrogens were removed from the ligand, and their partial atomic charges were united with the bonded carbon atoms. The docking runs were performed using the Lamarckian genetic algorithm with grid sizes of 60 × 60 × 60 (grid spacing 0.375 Å), yielding 10 docked conformations. During the docking computation, free rotation was allowed around the two C-N aliphatic bonds. Three binding energy terms were taken into account in the docking step: the van der Waals interaction represented as a Lennard-Jones dispersion–repulsion term, the hydrogen bonding term, and the Coulombic electrostatic potential. The resulting 20,000 poses for NCP were analyzed by grouping them into clusters with similar ligand orientations.

Other Software Used

Molecular illustrations were created with UCSF Chimera (Pettersen et al., 2004). Ramachandran plot was calculated in Rampage (Lovell et al., 2003). Secondary structure was recognized with ProMotif (Hutchinson and Thornton, 1996) within PDBsum server (de Beer et al., 2014). Sequence alignment was performed in CLUSTAL W (Thompson et al., 1994), and edited in BioEdit (Hall, 1999).

Results and Discussion

MtCPA Forms Helical Octamers

The polypeptide chain of MtCPA contains 301 amino acids and its calculated molecular weight is 33.8 kDa. MtCPA crystallizes in P21212 space group, with two octamers (chains A-H and I-P) as the asymmetric unit. In each of the structures presented herein, the octamer-flanking monomers (subunits A and H in the first octamer, and I and P in the second) present higher degree of flexibility than the inner subunits of the octamers. This is most probably due to lack of intermolecular contacts, which allows for higher conformational fluctuations. As a result, the electron density maps for the flanking protein subunits (monomers A, H, I, P) were not clear enough to model ligand molecules, and the ligands were placed for 12 out of 16 protein chains (B–G and J–O).

CPAs show high degree of similarity, especially among plant species (Figure 2). Therefore, many conclusions, inferred from the presented structures, may be extrapolated to other CPA enzymes. The octameric quaternary structure in the crystal lattice of MtCPA is in agreement with the assembly reported, based on native gel electrophoresis, for the very close ortholog from A. thaliana (85% identity, 92% similarity) (Piotrowski et al., 2003). Based on the crystal structure, MtCPA octamers resemble an incomplete left-handed helical twist with an outer diameter of about 110 Å (Figure 3). The helical octamer surrounds a central void of 20 Å diameter. MtCPA octamer can be divided into four symmetric dimers that are shifted by about 30 Å along the long axis of adjacent dimer(s). The gap between the first and the last dimer within the octamer is approximately 10 Å. The dimers present αββααββα topology, and are formed by two monomers of αββα sandwich fold, which is very characteristic for the members of nitrilase superfamily (Nakai et al., 2000; Raczynska et al., 2011). To form a dimer, MtCPA monomers mutually swap their C-terminal fragments from His275 to Leu301 (Figure 4) on the inner side of the octamer. The C-terminal swap anchors the monomers to each other in an arm-to-arm manner, sturdily enhancing the monomer-monomer interactions. Furthermore, residues Asp295:Leu301 do not interact with a dimer mate, but instead increase the dimer-dimer interfaces in all but first (A/B and I/J) dimers in each octamer.

FIGURE 2
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FIGURE 2. Sequence alignment of selected nitrilase enzymes. UniProt accession numbers are given in square brackets, and the values in per cent indicate sequence identity to MtCPA. Six first sequences correspond to CPA enzymes from: MtCPA [G7ITU5]; Glycine max, (GmCPA) [I1M4B9] 94%; Solanum tuberosum, (StCPA) [Q3HVN1] 86%; Arabidopsis thaliana, (AtNLP1/CPA) [B9DGV9] 85%; Os Indica group putative protein (OsCPA) [A2X5P5] 82%, Pseudomonas aeruginosa CPA (PaerCPA) [A6UY94] 64%. The other three sequences belong to protein structures described in this manuscript: Pyrococcus abyssi Nitrilase (PaNit) [Q9UYV8] 35%; Drosophila melanogaster β-Alanine Synthase without 60 N-terminal residues (DmβAS) [Q9VI04] 31% and Helicobacter pylori Formamidase (HpAmiF) [M3MZ63] 27%. Numbering above the sequences and annotation of the secondary structure elements (α helices, red bars; η 310 helices, pink; β strands, blue) corresponds to MtCPA. Residues are color-coded by type, and E48, K121, E132, C158 and E187 in MtCPA sequence are highlighted in yellow.

FIGURE 3
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FIGURE 3. MtCPA octamer. Surface of each protein subunit (capital letters, A–H) is colored differently. Dimensions are given in Å.

FIGURE 4
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FIGURE 4. Detailed view on an isolated MtCPA dimer with annotation of the secondary structure. Numbering of helices is consecutive, regardless of their type, and η indicate 310 helices. The reaction intermediate, DHMP and the active Cys158 are pictured to visualize the enzymatic reaction venue. Protein chains C (light blue) and D (salmon) are shown.

The oligomerization state varies among the nitrilases, although they all present a common architecture of αββααββα dimers, with swapped C-terminal fragments analogical to those observed in MtCPA. The length of the swapped fragments varies among proteins with available structures from nitrilase family, from short swap of as little as 10-residue fragment (Kumaran et al., 2003) to longer of about 70 residues (Agarkar et al., 2006). The quaternary assemblies of nitrilases are universally composed of even number of protein subunits. More precisely, the reported functional oligomers vary from dimers (Barglow et al., 2008; Liu et al., 2013), tetramers (Wang et al., 2001), hexamers (Agarkar et al., 2006), octamers, like MtCPA or β-alanine synthase from Drosophila Melanogaster (DmβAS) (Lundgren et al., 2008), through higher tube-like spiral multimers (Jandhyala et al., 2003; Sewell et al., 2003; Thuku et al., 2007).

In the PDB, one protein of the nitrilase family, DmβAS (Lundgren et al., 2008) (PDB ID: 2VHI), presents helically shaped octamers that resemble those formed by MtCPA. Even though the structures of MtCPA and DmβAS proteins present a similar assembly of the dimers at the first glance, the twist of the MtCPA octamer is more coiled. In contrast, the “uncoiled” DmβAS octamer has a diameter of approx. 120 Å, void of ≈ 30 Å and 65–70 Å pitch (rise along the axis per turn), whereas the corresponding values for MtCPA are: 110, 20, and 45 Å, with the latter value being only theoretical because the pitch of an incomplete helix is virtual. Authors report that DmβAS can freely form higher helical oligomers by attachment of further dimers to the octamer. In contrast, the helix pitch of MtCPA is too small to accommodate another dimer (≈ 75 Å along the long axis), and the addition of further dimers would either create severe steric clashes or force significant structural rearrangements (uncoiling) of the octamer. Consistently, the flanking dimers of the MtCPA octamer are separated by only a 10 Å gap, much narrower than in the DmβAS octamer. In DmβAS, the gap between the first and last dimer is almost 40 Å, which is sufficient to accommodate additional dimer, necessary for the formation of the theoretically infinite helical assembly.

Complexes with: The Reaction Intermediate, CAD and the Structure of MtCPA-C158S Mutant and Its Complex with PUT

The structures of wild-type MtCPA, crystallized in the presence of PUT and CAD in the solution, were determined at 1.97 and 2.19 Å resolution, respectively. Inspection of the electron density maps, representing the structure of MtCPA cocrystallized with PUT, brought unexpected, but very informative results. Instead of linear PUT, the reaction intermediate, DHMP, was observed in the active site (Figure 5A). More interestingly, DHMP was covalently bound to the catalytic Cys158. There are two conceivable scenarios of the DHMP adduct formation during crystallization. It is possible that PUT reacts with carbon dioxide (or carbonic acid) in solution, outside the catalytic site of the enzyme, for it is known that primary amines react with CO2 in aqueous solution (Penny and Ritter, 1983; McCann et al., 2009). The resulting N-carbamicputrescine (with carboxylic COO- group attached to one of the PUT amines) may enter the active site and, similarly to the NCP, most likely is susceptible to the nucleophilic attack of the Cys158. The DHMP covalent adduct is stabilized by placement of one of its oxygen atoms within the oxyanion hole, created by Nζ of Lys121 and the backbone N of Trp159 (see Active Site and the Reaction Mechanism). The other scenario of events, which might lead to the covalent enzyme-DHMP adduct in the crystallization drop, involves an initial reaction of carbon dioxide (or carbonic acid) with the active Cys158. To our judgment, however, this situation is much less likely for two reasons. Firstly, the covalent C-N bond in that case would need to result from a nucleophilic attack of N atom of PUT on the S-bound carboxyl C, which is very questionable. Secondly, if the second scenario was true, one would expect a similar state in the structure of MtCPA cocrystallized with CAD, because nothing should prevent the Cys158 carboxylation in the first place. In that instance, there would be not enough room to bind entire CAD molecule. This is not the case, and we do indeed observe CAD in the active site (Figure 5B). It is, of course, possible that CAD molecules in solution also form CO2 adducts, but due to steric clashes (see Substrate Specificity), they cannot be recruited to the catalytic site, meanwhile non-modified CAD molecules can. CAD in MtCPA complex reaches deeper than PUT into the catalytic pocket, however, due to presence of sulfhydryl group of Cys158 it bends toward Glu132.

FIGURE 5
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FIGURE 5. Ligand binding by MtCPA (A,B) and MtCPA C158S mutant (C,D). In each panel protein subunits C (blue C atoms) and D (salmon) are shown whereas the ligands: DHMP in (A); CAD (B); PUT (C) and GOL (D) are in gray. Green meshes visualize omit electron density maps contoured at 5 σ level around ligands. Dashed black lines indicate hydrogen bonds. Semitransparent residues in (B–D) do not interact with ligands, and are depicted for comparison only.

The crystal structure of wild-type MtCPA without addition of any ligands was determined at 2.55 Å resolution (data not shown). Unfortunately, the electron density maps for the content of the catalytic site were unclear, and represented most probably disordered ingredients of the crystallization solution, GOL, and partially oxidized Cys158. Combined with the rather poor data resolution, we were not able to unambiguously interpret the content of the active site of “unliganded” wild-type MtCPA, and we do not report this structure herein. Instead, we decided to construct the MtCPA-C158S mutant. Substitution of sulfhydryl with hydroxyl group preserved binding properties of residue 158 but strongly diminished its reactivity. The structure of unliganded MtCPA-C158S, determined at 2.39 Å resolution, presented significantly lower noise in the electron density maps around the active site when compared to the unliganded wild-type MtCPA. This improvement allowed to identify the ligand bound inside the active site as GOL (Figure 5C). However, GOL does not penetrate deep inside the pocket and presents no direct interactions with either of the residues from catalytic triad. Instead, it is hydrogen-bonded with the side chain oxygen of Glu187.

The crystal structure of MtCPA-C158S mutant cocrystallized with PUT clearly shows the ligand without any modifications (Figure 5D). In this case, the absence of nucleophilic sulfur prevents from the formation of covalent bond between DHMP and residue 158. In fact, PUT in MtCPA-C158S complex does not interact directly with the residue 158, but creates water-mediated hydrogen bond with the hydroxyl group of Ser158 instead.

Active Site and the Reaction Mechanism

Each MtCPA monomer contains a cavity, which is accessible from the outer surface of MtCPA octamer and, in its depth, comprises the active site. In order to present the active sites in a clear manner, we divide the MtCPA cavities to four parts, each buried deeper in the protein core: (i) the entrance preceding the genuine active site; (ii) the tail amine-binding region, which binds the non-reacting amine group of PA; (iii) the non-polar section, interacting with the ligand aliphatic fragment; and (iv) the catalytic triad, which performs the reaction. The cavities are in a very close proximity to the neighboring protein subunits, with the exception of the outer monomers A, H, I, and P that only have a single neighbor. The entrances to the funnel-like catalytic cavities are actually shaped not only by the amino acids from the protein subunit to which a particular site belongs, but are also fenced by protein chains of its immediate neighbor(s) (Figure 6). Moreover, each dimer-mate subunit surrounds a larger fragment of the active site entrance than the protein chain from the neighboring dimer.

FIGURE 6
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FIGURE 6. The active site of MtCPA. (A) View along the entrance to the cavity which contains the active site, and the reaction intermediate, DHMP inside. Protein subunits B (yellow), C (light blue) and D (salmon) are shown. (B) Detailed mode of interaction of MtCPA with DHMP. Dashed lines indicate hydrogen-bonded atoms. Hydrogen bonds mediated by more than one water molecule are omitted for clarity. Cα atoms of interacting residues are shown as balls. The protein surface (semitransparent, C and D) is clipped to show the maximum vista over the binding cavity.

Glu187, Asp190, together with several carbonyl oxygens of Trp277 (asterisk indicates a residue that belongs to dimer-mate subunit), Cys276, Asp126 and Pro128 are responsible for the negative potential localized around the active site (Figure 6A). Most probably, they attract the positively charged NCP, when it penetrates its way through the cavity. Walls of the middle section of the active site are composed of the side chains of: Tyr130, Tyr54, Pro125, Trp159, Trp162, Ile184, Ala183, and by Trp277 from the swapped C-terminal fragment (Figure 6B). In this manner, MtCPA provides the hydrophobic milieu of the central section of the active pocket. This fragment is, therefore, perfectly adapted to bind the aliphatic fragment of the substrate, NCP by hydrophobic interactions.

As in other nitrilases, the substrate hydrolysis is carried out by the catalytic triad, composed in MtCPA of Glu48 (proton acceptor), Lys121 (proton donor) and Cys158 (nucleophile). These three residues are placed deep inside the narrow part of the active site. The nucleophilic Cys, as in any other nitrilase-like protein, is positioned at the apex of the nucleophile elbow (Kumaran et al., 2003), formed in MtCPA by β7-turn-η6 motif, and its tightness enhances the nucleophilic character of Cys158 by enforcing energetically unfavorable conformation. The nucleophilic character of the active Cys158 is additionally fortified by two glutamates, Glu48 and Glu132, which attract the sulfhydryl proton. Both glutamates, i.e., Glu48, as the member of the catalytic triad, but also Glu132 are highly conserved among nitrilase superfamily. Most probably, this pair attracts the NH2 group of the NCP, therefore, properly orients the carbamoyl carbon of the substrate for the nucleophilic attack by Cys158. Moreover, Glu48 and Glu132 affect the closest environment of Lys121 and preserve its positive charge, crucial for the hydrolysis.

The hydrolysis of NCP by MtCPA most likely follows a mechanism similar at first stages to the proposed earlier for Helicobacter pylori formamidase (HpAmiF) (Hung et al., 2007), but after creation of the oxyanion geminal diol intermediate (see below), it carries on in its own way. Briefly, activated Sγ of Cys158 performs nucleophilic attack on the carbamoyl C atom of the substrate, creating the covalent, tetrahedral (geometry concerns the initially planar C atom, which ultimately leaves as HCO3) diaminothioalcoholate intermediate (Figure 7). The generated oxyanion is stabilized by the oxyanion hole, formed by Nζ of Lys121 and backbone N of Trp159, similarly to the case reported for Pyrococcus abyssi nitrilase (PaNit) (Raczynska et al., 2011). Subsequently, the amino group of the intermediate accepts a proton, donated by Glu48, and leaves as the first by-product, ammonia, resulting in the planar S-acyl intermediate-enzyme complex, which is hydrated to yield the tetrahedral oxyanionic geminal diol (present in the crystal structure of MtCPA/DHMP complex). Then, most probably, the water molecule tethered to O𝜀 of Gln161 and N𝜀 of Trp162 is added to the intermediate, and, in an apparently concerted manner, C-S and C-N bonds are cleaved, which results in the release of PUT and the second by-product, HCO3-.

FIGURE 7
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FIGURE 7. A scheme of enzymatic hydrolysis of NCP to PUT. Enz-S-DHMP indicates the covalent complex with N-(dihydroxymethyl)putrescine, observed in the MtCPA/DHMP structure.

Substrate Specificity

Enzymatic assays on CPA enzymes from At (Piotrowski et al., 2003) and Pseudomonas aeruginosa (PaerCPA, Nakada and Itoh, 2003) show that CPAs are highly active only against NCP. Plant AtCPA showed no activity toward substrates of other nitrilase-like enzymes, e.g., amino acids, N-Carbamoyl-β-alanine, agmatine. Also, the bacterial PaerCPA very poorly hydrolyzed both longer and shorter substrates in comparison to NCP: N-carbamoylcadaverine and N-carbamoyldiaminopropane, respectively.

We addressed the question of structural features that are responsible for such narrow substrate specificity of CPA enzymes. The comparison of the product (PUT), its longer analog (CAD) and the intermediate (DHMP) bound within the active site of MtCPA highlights key elements of the active site architecture, which determine the enzyme preference for NCP (Figure 8). All bound amines, CAD, PUT and DHMP, present the same hydrogen bond between terminal amine group and the side chain oxygen of Glu187. Additionally, these amino groups create two water-mediated hydrogen bonds with carbonyl oxygens of Asp126, Trp277, and mediated by two waters hydrogen bonds with Pro128 and Cys276. Glu187, conserved in CPA enzymes, prevents from substrate mismatch, and stabilizes substrate position within the active site. Moreover, the position of negatively charged Glu187 at the active site entrance determines both the charge and length of the bound substrate. Longer or shorter molecules than NCP, would not be able to create a hydrogen bond with the oxygen of Glu187, and/or would collide with other parts of the active site.

FIGURE 8
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FIGURE 8. Substrate specificity of MtCPA. The ligands (semitransparent) inside the cavity originate from MtCPA/DHMP complex (green); MtCPA/CAD (yellow); MtCPA-C158S/PUT (magenta). GOL molecule (black wires) is superposed from MtCPA-C158S unliganded structure. Interacting amino acid residues and hydrogen-bonding network (dashed black lines) are shown for MtCPA/DHMP complex only, but their locations are preserved in MtCPA/CAD and MtCPA-C158S/PUT complexes as well. Asterisks () indicate amino acid residues that belong to dimer-mate subunit. Interactions mediated by more than two water molecules (red balls) are omitted for clarity.

The pocket presents very narrow and highly hydrophobic middle section, which excludes bulky substrates form binding. It also limits the spectrum of possible substrates to those which have an unbranched aliphatic fragment of four carbon atoms. From the MtCPA/CAD complex, we can assume that longer substrates than NCP, such as N-carbamoylcadaverine, would not obtain stable conformation inside the active site. Although CAD is able to interact via hydrogen bond with Glu187 at the entrance of the pocket, similarly to PUT and DHMP, deep inside the cleft CAD passes by the Sγ of Cys158 and bends toward the pair of glutamates. Thus, this would not leave enough space for the carbamoyl moiety of such longer substrate. In other words, the proper orientation of N-carbamoylcadaverine, with the preservation of the hydrogen bond with the Glu187 side chain is impossible due to steric clashes either with the catalytic triad or with the residues in the middle section of the pocket.

The commercial availability of NCP is extremely limited, therefore, during our studies, we attempted to obtain complexes with other ligands, such as urea, sarcosine, L-lysine, L-arginine, which would mimic the substrate. Unfortunately, their complexes with neither wild-type MtCPA nor its C158S mutant allowed to unambiguously identify any other ligand of interest within the active site, except for those presented in this paper.

Proposed Secondary Binding Site

As it was shown by Piotrowski et al. (2003), the hydrolysis of NCP by CPA from A. thaliana does not follow the Michaelis–Menten kinetics. Instead, in the excess of substrate, an accelerating mechanism is triggered. Since PAs are linked with the plants response to stress factors, this phenomenon may actually be significant in vivo. The positive allosteric regulation was found also in other nitrilase-like proteins, β-alanine synthases (Tamaki et al., 1987; Matthews et al., 1992; Sakamoto et al., 2001; Lundgren et al., 2008). In these enzymes, the mechanism was attributed to the change of oligomerization caused by increasing substrate concentration, rather than to the existence of an allosteric regulatory site (Matthews et al., 1992). However, in MtCPA, assuming that it also follows the Hill kinetics, due to disabled formation of higher oligomers, a different mechanism may control the enzyme behavior.

The architecture of close neighborhood of the catalytic site shows a solvent/cytoplasm accessible niche near the substrate binding pocket. In every structure presented herein, this niche is occupied by a GOL molecule. Considering the fact that in the MtCPA-C158S mutant structure, GOL enters the active site, and mimics the substrate or product, the niche-bound GOL quite likely might represent the secondary binding site. In that case, in higher concentration of NCP, this site might be occupied by the substrate. Docking simulation seems to support this hypothesis. In fact, the carbamoyl moiety of the docked substrate, NCP, significantly overlaps with the GOL-binding site from the presented here complexes (Figure 9). The substrate is situated in the niche with the carbamoyl moiety aiming at the entrance to the active site. In the predicted alternative binding site, NCP, would form three hydrogen bonds with Asp194, His198 and Glu248. The calculated binding energy of the secondary binding site is -3.6 kcal mol-1, whereas the corresponding value for the genuine catalytic cavity equals -5.8 kcal mol-1. It is, therefore, suggestive that the substrate affinity is significantly lower in the alternative binding site, nonetheless, still within a reasonable range.

FIGURE 9
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FIGURE 9. The proposed alternative substrate-binding site. The substrate (ball-and-sticks, green C atoms) was docked at the location where a GOL molecule (magenta) is present universally in all presented crystal structures. Note that the carbamoyl moiety of the substrate partially overlaps with the GOL position. The reaction intermediate, DHMP (ball-and-sticks, gray), bound in the catalytic center is shown to visualize the structural proximity of the two sites. Dashed black lines indicate possible hydrogen bonds with Asp194, His198 and Glu248. The surfaces of the two dimer-forming protein subunits are color-coded red and blue.

At this point, however, the mechanism of allosteric regulation remains unrevealed, for it appears that binding of the second NCP molecule, should neither directly facilitate binding of the substrate within the active site, nor it should impact the catalytic triad. It is possible that the alternative NCP binding location represents a standby spot for substrate molecule. Even though it would not be an allosteric regulation of the enzyme activity per se, it would mitigate the delay needed for the substrate diffusion into the active site. By far, it is merely a speculation, and many additional experiments are required to validate this hypothesis, however, it is worth to mention that a standby substrate position was reported, e.g., for tyrosine phosphatase from Selenomonas ruminantium (Puhl et al., 2007), unrelated to CPA proteins.

Conclusions, Physiological Significance and Future Outlook

This study was focused on the structural characterization of CPA from the model legume plant, M. truncatula. The octameric MtCPA enzyme is assembled into an incomplete helical twist, made by four tight dimers with swapped C-termini. This dimeric αββααββα organization is highly conserved among nitrilase-like enzymes, however, the analogical octameric assembly was observed only in DmβAS (Lundgren et al., 2008).

The octameric structure of plant CPAs, reported previously for A. thaliana (Piotrowski et al., 2003) and herein for M. truncatula brings up a fundamental question of physiological benefit from forming high oligomers. The role of PUT in response to abiotic stresses (mentioned in the Introduction), such as high salinity, drought and/or thermal extrema, could provide a conceivable answer. Assembling into higher oligomers undoubtedly increases enzyme’s tolerance to adverse conditions, for a smaller portion of the protein surface is exposed toward the cytoplasm and, therefore, is less susceptible to changing environment. A similar rationale was anticipated to explain oligomerization of other abiotic-stress-related plant proteins, which form ring-like decamers, δ1-pyrroline-5-carboxylate reductases (Forlani et al., 2015).

N-carbamoylputrescine amidohydrolases are enzymes highly specific towards NCP (Piotrowski et al., 2003), and the architecture of the MtCPA catalytic cavity, formed as a deep pocket with broadened entrance, explains this phenomenon. The entrance and its middle section is built with a contribution of the residues from neighboring monomers Cys276 and Trp277. Two characteristic features influence the substrate specificity of MtCPA: the narrow and hydrophobic channel in the middle section of the catalytic cavity (Tyr130, Tyr54, Pro125, Trp159, Trp162, Ile184, Ala183 and Trp277 from dimer mate) and Glu187, placed at the entrance, the key residue responsible for the proper substrate orientation inside the active site. The catalytic triad at the bottom of the cavity is composed of Glu48, Lys121 and Cys158. Glu48, the proton acceptor, in the cooperation with Glu132 enhances the nucleophilic character of Cys158 and maintains the proper charge of Lys121, the proton donor. Lys121, together with backbone N of Trp159 forms the oxyanion hole, which stabilizes the intermediate state during NCP hydrolysis. Cys158, placed at the apex of the nucleophile elbow, formed in MtCPA by β7-turn-η6 motif, is responsible for the nucleophilic attack on the substrate, and creation of the covalent intermediate-enzyme complex. The catalytic water molecule, which performs subsequent nucleophilic attack on the intermediate, is stored within the active site in a small niche, near the catalytic triad. This water is hydrogen-bonded to the side chains of Gln161 and Trp162. The reaction leads to the breakage of two covalent bonds of the substrate, which ends with the release of PUT, ammonia and carbon dioxide. Presented here indication of the key residues, responsible for specificity and activity of MtCPA, sheds new light on CPA enzymes overall. Any future in-depth physiological study of CPAs can be more rational, as the research can benefit, or even directly arise from the structural knowledge presented herein.

The crystallographic analysis of the complexes of MtCPA and its C158S mutant confirmed high affinity of their active sites for ligands, which were either absorbed from crystallization solution (GOL), or intentionally added to obtain MtCPA complexes (PUT and CAD). Interestingly, in the complex of the wild-type MtCPA, obtained by the cocrystallization with PUT, the reaction intermediate, DHMP, was covalently bound to the active Cys158, inside the active site instead of PUT. DHMP adduct was most probably formed as the result of the reaction of the amine group of PUT with carbon dioxide, absorbed by the crystallization drop, followed by nucleophilic attack of the active Cys158. This showed that the oxyanion hole, next to the MtCPA catalytic triad, is able to stabilize the otherwise labile geminal diol. It would be very interesting to see whether a similar scenario could be relevant in planta, that is, if CO2 to a significant extent reacts with PUT in the cytoplasm and (as carbamic acid) enters the catalytic cavity of MtCPA. If so, the enzyme activity would be modulated by CO2 concentration, which would give another link between PAs and plant stress response.

Several members of nitrilase superfamily have been previously reported to exert enzymatic mechanism suggesting cooperative binding. Due to lack of a candidate secondary substrate-binding position, for most of them this behavior was associated with changes of the oligomerization state. MtCPA, however, is not able to change the oligomerization state, as its octamers are formed in a very coiled manner. We examined MtCPA structure to indicate a secondary substrate-binding site. The analysis led to designation of the conserved (in MtCPA structures) GOL binding location as the potential alternative substrate binding site. This hypothesis was supported by docking experiment, which indicated that the substrate may indeed bind also in a niche, with carbamoyl moiety of the docked NCP partially overlapping the GOL binding site. This venue is very close to the entrance of the active site, but separated from the catalytic triad. However, with present data we are not able to unambiguously determine the activity-accelerating mechanism linked to the alternative binding site. We may suppose that MtCPA might not be allosterically regulated per se, but rather own a site, where the substrate can standby, prior to entering the catalytic site. In that case, the turnover rate of the enzyme would be increased, as the delay needed for the substrate to diffuse in the cavity would be alleviated if it was bound right next to the entrance. This hypothesis, however, needs to be verified using parallel functional and structural approaches, nonetheless, it sketches a perspective for future studies of CPA enzymes. From the physiological perspective, accelerating mechanism is very beneficial, as it triggers increased enzyme activity when it is most needed, bypassing regulatory mechanisms of transcription and translation. During abiotic and biotic stresses as well as in the course of nodulation, when the demand for PAs is aggravated, plant can produce sufficient amount of PUT without engaging the protein synthesis machinery to deliver more molecules of CPA, but instead simply providing more NCP.

Accession Numbers

Coordinates and structure factors of the related structures were deposited in the PDB: MtCPA/DHMP complex, 5H8I; MtCPA/CAD, 5H8J; MtCPA-C158S mutant, 5H8K; MtCPA-C158S/PUT, 5H8L.

Author Contributions

BS produced the protein and solved the crystal structures. BS, MR, and ZD analyzed the data. MM performed docking calculations. MR and BS wrote the manuscript.

Conflict of Interest Statement

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Acknowledgments

This project was supported in part by the Intramural Research Program of the NCI, Center for Cancer Research. Diffraction data were collected at the SER-CAT beamline 22-ID at the Advanced Photon Source, Argonne National Laboratory, supported by the US Department of Energy, Office of Science, Office of Basic Energy Sciences under Contract W-31-109-Eng-38. The research was conducted during the Ph.D. scholarship of B.S. (2014/12/T/ST5/00136) financed by Polish National Science Centre. We gratefully acknowledge Miroslawa Dauter for the valuable advice and assistance during crystallization of MtCPA.

Abbreviations

ADC, arginine decarboxylase; AIH, agmatine iminohydrolase; At, Arabidopsis thaliana; CAD, cadaverine; cDNA, complementary DNA; CPA, N-carbamoylputrescine amidohydrolase; DmβAS, Drosophila Melanogaster β-alanine synthase; DHMP, N-(dihydroxymethyl)putrescine; GOL, glycerol; Gm, Glycine max; HpAmiF, Helicobacter pylori formamidase; IPTG, isopropyl-β-D-thiogalactopyranoside; Mt, Medicago truncatula; NCP, N-carbamoylputrescine; ODC, ornithine decarboxylase; Os, Oryza sativa; PA, polyamine; Paer, Pseudomonas aeruginosa; PaNit, Nitrilase from Pyrococcus abyssi; PCR, polymerase chain reaction; PDB, Protein Data Bank; PUT, putrescine; SPD, spermidine; SPM, spermine; St, Solanum tuberosum; TCEP, tris(2-carboxyethyl)phosphine; TEV, Tobacco Etch Virus.

References

Agarkar, V. B., Kimani, S. W., Cowan, D. A., Sayed, M. F., and Sewell, B. T. (2006). The quaternary structure of the amidase from Geobacillus pallidus RAPc8 is revealed by its crystal packing. Acta Crystallogr. Sect. F Struct. Biol. Cryst. Commun. 62, 1174–1178. doi: 10.1107/S1744309106043855

PubMed Abstract | CrossRef Full Text

Alcazar, R., Planas, J., Saxena, T., Zarza, X., Bortolotti, C., Cuevas, J., et al. (2010). Putrescine accumulation confers drought tolerance in transgenic Arabidopsis plants over-expressing the homologous Arginine decarboxylase 2 gene. Plant Physiol. Biochem. 48, 547–552. doi: 10.1016/j.plaphy.2010.02.002

PubMed Abstract | CrossRef Full Text | Google Scholar

Bachrach, U. (2010). The early history of polyamine research. Plant Physiol. Biochem. 48, 490–495. doi: 10.1016/j.plaphy.2010.02.003

PubMed Abstract | CrossRef Full Text | Google Scholar

Barglow, K. T., Saikatendu, K. S., Bracey, M. H., Huey, R., Morris, G. M., Olson, A. J., et al. (2008). Functional proteomic and structural insights into molecular recognition in the nitrilase family enzymes. Biochemistry 47, 13514–13523. doi: 10.1021/bi801786y

PubMed Abstract | CrossRef Full Text | Google Scholar

Berman, H. M., Westbrook, J., Feng, Z., Gilliland, G., Bhat, T. N., Weissig, H., et al. (2000). The protein data bank. Nucleic Acids Res. 28, 235–242. doi: 10.1093/nar/28.1.235

CrossRef Full Text | Google Scholar

Bork, P., and Koonin, E. V. (1994). A new family of carbon-nitrogen hydrolases. Protein Sci. 3, 1344–1346. doi: 10.1002/pro.5560030821

PubMed Abstract | CrossRef Full Text | Google Scholar

Brunger, A. T. (1992). Free R value: a novel statistical quantity for assessing the accuracy of crystal structures. Nature 355, 472–475. doi: 10.1038/355472a0

PubMed Abstract | CrossRef Full Text | Google Scholar

Capell, T., Bassie, L., and Christou, P. (2004). Modulation of the polyamine biosynthetic pathway in transgenic rice confers tolerance to drought stress. Proc. Natl. Acad. Sci. U.S.A. 101, 9909–9914. doi: 10.1073/pnas.0306974101

PubMed Abstract | CrossRef Full Text | Google Scholar

Chen, C. Y., Chiu, W. C., Liu, J. S., Hsu, W. H., and Wang, W. C. (2003). Structural basis for catalysis and substrate specificity of Agrobacterium radiobacter N-carbamoyl-D-amino acid amidohydrolase. J. Biol. Chem. 278, 26194–26201. doi: 10.1074/jbc.M302384200

PubMed Abstract | CrossRef Full Text | Google Scholar

Chen, V. B., Arendall, W. B., Headd, J. J., Keedy, D. A., Immormino, R. M., Kapral, G. J., et al. (2010). MolProbity: all-atom structure validation for macromolecular crystallography. Acta Crystallogr. D Biol. Crystallogr. 66, 12–21. doi: 10.1107/S0907444909042073

PubMed Abstract | CrossRef Full Text | Google Scholar

de Beer, T. A., Berka, K., Thornton, J. M., and Laskowski, R. A. (2014). PDBsum additions. Nucleic Acids Res. 42, D292–D296. doi: 10.1093/nar/gkt940

PubMed Abstract | CrossRef Full Text | Google Scholar

Do, P. T., Drechsel, O., Heyer, A. G., Hincha, D. K., and Zuther, E. (2014). Changes in free polyamine levels, expression of polyamine biosynthesis genes, and performance of rice cultivars under salt stress: a comparison with responses to drought. Front. Plant Sci. 5:182. doi: 10.3389/fpls.2014.00182

PubMed Abstract | CrossRef Full Text | Google Scholar

Efrose, R. C., Flemetakis, E., Sfichi, L., Stedel, C., Kouri, E. D., Udvardi, M. K., et al. (2008). Characterization of spermidine and spermine synthases in Lotus japonicus: induction and spatial organization of polyamine biosynthesis in nitrogen fixing nodules. Planta 228, 37–49. doi: 10.1007/s00425-008-0717-1

PubMed Abstract | CrossRef Full Text | Google Scholar

Emsley, P., Lohkamp, B., Scott, W. G., and Cowtan, K. (2010). Features and development of Coot. Acta Cryst. D 66, 486–501. doi: 10.1107/S0907444910007493

PubMed Abstract | CrossRef Full Text | Google Scholar

Forlani, G., Makarova, K. S., Ruszkowski, M., Bertazzini, M., and Nocek, B. (2015). Evolution of plant (1-pyrroline-5-carboxylate reductases from phylogenetic and structural perspectives. Front. Plant Sci. 6:567. doi: 10.3389/fpls.2015.00567

PubMed Abstract | CrossRef Full Text | Google Scholar

Fuell, C., Elliott, K. A., Hanfrey, C. C., Franceschetti, M., and Michael, A. J. (2010). Polyamine biosynthetic diversity in plants and algae. Plant Physiol. Biochem. 48, 513–520. doi: 10.1016/j.plaphy.2010.02.008

PubMed Abstract | CrossRef Full Text | Google Scholar

Fujihara, S., Abe, H., Minakawa, Y., Akao, S., and Yoneyama, T. (1994). Polyamines in nodules from various plant-microbe symbiotic associations. Plant Cell Physiol. 35, 1127–1134.

Google Scholar

Gill, S. S., and Tuteja, N. (2010). Polyamines and abiotic stress tolerance in plants. Plant Signal. Behav. 5, 26–33. doi: 10.4161/psb.5.1.10291

CrossRef Full Text | Google Scholar

Hall, T. A. (1999). BioEdit: a user-friendly biological sequence alignment editor and analysis program for Windows 95/98/NT. Nucl. Acids Symp. Ser. 41, 95–98.

Google Scholar

Hanfrey, C., Sommer, S., Mayer, M. J., Burtin, D., and Michael, A. J. (2001). Arabidopsis polyamine biosynthesis: absence of ornithine decarboxylase and the mechanism of arginine decarboxylase activity. Plant J. 27, 551–560. doi: 10.1046/j.1365-313X.2001.01100.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Hung, C. L., Liu, J. H., Chiu, W. C., Huang, S. W., Hwang, J. K., and Wang, W. C. (2007). Crystal structure of Helicobacter pylori formamidase AmiF reveals a cysteine-glutamate-lysine catalytic triad. J. Biol. Chem. 282, 12220–12229. doi: 10.1074/jbc.M609134200

PubMed Abstract | CrossRef Full Text | Google Scholar

Hutchinson, E. G., and Thornton, J. M. (1996). PROMOTIF–a program to identify and analyze structural motifs in proteins. Protein Sci. 5, 212–220. doi: 10.1002/pro.5560050204

PubMed Abstract | CrossRef Full Text | Google Scholar

Igarashi, K., and Kashiwagi, K. (2010). Modulation of cellular function by polyamines. Int. J. Biochem. Cell Biol. 42, 39–51. doi: 10.1016/j.biocel.2009.07.009

PubMed Abstract | CrossRef Full Text | Google Scholar

Illingworth, C., Mayer, M. J., Elliott, K., Hanfrey, C., Walton, N. J., and Michael, A. J. (2003). The diverse bacterial origins of the Arabidopsis polyamine biosynthetic pathway. FEBS Lett. 549, 26–30. doi: 10.1016/S0014-5793(03)00756-7

PubMed Abstract | CrossRef Full Text | Google Scholar

Jandhyala, D., Berman, M., Meyers, P. R., Sewell, B. T., Willson, R. C., and Benedik, M. J. (2003). CynD, the cyanide dihydratase from Bacillus pumilus: gene cloning and structural studies. Appl. Environ. Microbiol. 69, 4794–4805. doi: 10.1128/AEM.69.8.4794-4805.2003

PubMed Abstract | CrossRef Full Text | Google Scholar

Jimenez-Bremont, J. F., Marina, M., Guerrero-Gonzalez Mde, L., Rossi, F. R., Sanchez-Rangel, D., Rodriguez-Kessler, M., et al. (2014). Physiological and molecular implications of plant polyamine metabolism during biotic interactions. Front. Plant Sci. 5:95. doi: 10.3389/fpls.2014.00095

PubMed Abstract | CrossRef Full Text | Google Scholar

Kabsch, W. (2010). Xds. Acta Crystallogr. D Biol. Crystallogr. 66, 125–132. doi: 10.1107/S0907444909047337

PubMed Abstract | CrossRef Full Text | Google Scholar

Kamiab, F., Talaie, A., Khezri, M., and Javanshah, A. (2014). Exogenous application of free polyamines enhance salt tolerance of pistachio (Pistacia vera L.) seedlings. Plant Growth Regul. 72, 257–268. doi: 10.1007/s10725-013-9857-9

CrossRef Full Text | Google Scholar

Kasukabe, Y., He, L., Nada, K., Misawa, S., Ihara, I., and Tachibana, S. (2004). Overexpression of spermidine synthase enhances tolerance to multiple environmental stresses and up-regulates the expression of various stress-regulated genes in transgenic Arabidopsis thaliana. Plant Cell Physiol. 45, 712–722. doi: 10.1093/pcp/pch083

PubMed Abstract | CrossRef Full Text | Google Scholar

Kim, Y., Babnigg, G., Jedrzejczak, R., Eschenfeldt, W. H., Li, H., Maltseva, N., et al. (2011). High-throughput protein purification and quality assessment for crystallization. Methods 55, 12–28. doi: 10.1016/j.ymeth.2011.07.010

PubMed Abstract | CrossRef Full Text | Google Scholar

Klock, H. E., and Lesley, S. A. (2009). The Polymerase Incomplete Primer Extension (PIPE) method applied to high-throughput cloning and site-directed mutagenesis. Methods Mol. Biol. 498, 91–103. doi: 10.1007/978-1-59745-196-3_6

PubMed Abstract | CrossRef Full Text | Google Scholar

Kumar, R. R., Sharma, S. K., Rai, G. K., Singh, K., Choudhury, M., Dhawan, G., et al. (2014). Exogenous application of putrescine at pre-anthesis enhances the thermotolerance of wheat (Triticum aestivum L.). Indian J. Biochem. Biophys. 51, 396–406.

PubMed Abstract | Google Scholar

Kumaran, D., Eswaramoorthy, S., Gerchman, S. E., Kycia, H., Studier, F. W., and Swaminathan, S. (2003). Crystal structure of a putative CN hydrolase from yeast. Proteins 52, 283–291. doi: 10.1002/prot.10417

PubMed Abstract | CrossRef Full Text | Google Scholar

Laskowski, R. A., Macarthur, M. W., Moss, D. S., and Thornton, J. M. (1993). Procheck – a program to check the stereochemical quality of protein structures. J. Appl. Crystallogr. 26, 283–291. doi: 10.1107/S0021889892009944

CrossRef Full Text | Google Scholar

Liu, H., Gao, Y., Zhang, M., Qiu, X., Cooper, A. J., Niu, L., et al. (2013). Structures of enzyme-intermediate complexes of yeast Nit2: insights into its catalytic mechanism and different substrate specificity compared with mammalian Nit2. Acta Crystallogr. D Biol. Crystallogr. 69, 1470–1481. doi: 10.1107/S0907444913009347

PubMed Abstract | CrossRef Full Text | Google Scholar

Liu, J. H., Nada, K., Honda, C., Kitashiba, H., Wen, X. P., Pang, X. M., et al. (2006). Polyamine biosynthesis of apple callus under salt stress: importance of the arginine decarboxylase pathway in stress response. J. Exp. Bot. 57, 2589–2599. doi: 10.1093/jxb/erl018

PubMed Abstract | CrossRef Full Text | Google Scholar

Liu, J. H., Wang, W., Wu, H., Gong, X., and Moriguchi, T. (2015). Polyamines function in stress tolerance: from synthesis to regulation. Front. Plant Sci. 6:827. doi: 10.3389/fpls.2015.00827

PubMed Abstract | CrossRef Full Text | Google Scholar

Long, F., Vagin, A. A., Young, P., and Murshudov, G. N. (2008). BALBES: a molecular-replacement pipeline. Acta Crystallogr. D Biol. Crystallogr. 64, 125–132. doi: 10.1107/S0907444907050172

PubMed Abstract | CrossRef Full Text | Google Scholar

Lovell, S. C., Davis, I. W., Arendall, W. B. III, de Bakker, P. I., Word, J. M., Prisant, M. G., et al. (2003). Structure validation by Calpha geometry: phi,psi and Cbeta deviation. Proteins 50, 437–450. doi: 10.1002/prot.10286

PubMed Abstract | CrossRef Full Text | Google Scholar

Lundgren, S., Lohkamp, B., Andersen, B., Piskur, J., and Dobritzsch, D. (2008). The crystal structure of beta-alanine synthase from Drosophila melanogaster reveals a homooctameric helical turn-like assembly. J. Mol. Biol. 377, 1544–1559. doi: 10.1016/j.jmb.2008.02.011

PubMed Abstract | CrossRef Full Text | Google Scholar

Martin, W., Rujan, T., Richly, E., Hansen, A., Cornelsen, S., Lins, T., et al. (2002). Evolutionary analysis of Arabidopsis, cyanobacterial, and chloroplast genomes reveals plastid phylogeny and thousands of cyanobacterial genes in the nucleus. Proc. Natl. Acad. Sci. U.S.A. 99, 12246–12251. doi: 10.1073/pnas.182432999

PubMed Abstract | CrossRef Full Text | Google Scholar

Martin-Tanguy, J. (2001). Metabolism and function of polyamines in plants: recent development (new approaches). Plant Growth Regul. 34, 135–148. doi: 10.1023/A:1013343106574

CrossRef Full Text | Google Scholar

Matthews, M. M., Liao, W., Kvalnes-Krick, K. L., and Traut, T. W. (1992). beta-Alanine synthase: purification and allosteric properties. Arch. Biochem. Biophys. 293, 254–263. doi: 10.1016/0003-9861(92)90393-B

CrossRef Full Text | Google Scholar

McCann, N., Phan, D., Wang, X. G., Conway, W., Burns, R., Attalla, M., et al. (2009). Kinetics and mechanism of carbamate formation from CO2(aq), carbonate species, and monoethanolamine in aqueous solution. J. Phys. Chem. A 113, 5022–5029. doi: 10.1021/jp810564z

PubMed Abstract | CrossRef Full Text | Google Scholar

Minocha, R., Majumdar, R., and Minocha, S. C. (2014). Polyamines and abiotic stress in plants: a complex relationship. Front. Plant Sci. 5:175. doi: 10.3389/fpls.2014.00175

PubMed Abstract | CrossRef Full Text | Google Scholar

Moriarty, N. W., Grosse-Kunstleve, R. W., and Adams, P. D. (2009). electronic Ligand Builder and Optimization Workbench (eLBOW): a tool for ligand coordinate and restraint generation. Acta Cryst. D 65, 1074–1080. doi: 10.1107/S0907444909029436

PubMed Abstract | CrossRef Full Text | Google Scholar

Morris, G. M., Huey, R., Lindstrom, W., Sanner, M. F., Belew, R. K., Goodsell, D. S., et al. (2009). AutoDock4 and AutoDockTools4: automated docking with selective receptor flexibility. J. Comput. Chem. 30, 2785–2791. doi: 10.1002/jcc.21256

PubMed Abstract | CrossRef Full Text | Google Scholar

Mostofa, M. G., Yoshida, N., and Fujita, M. (2014). Spermidine pretreatment enhances heat tolerance in rice seedlings through modulating antioxidative and glyoxalase systems. Plant Growth Regul. 73, 31–44. doi: 10.1007/s10725-013-9865-9

CrossRef Full Text | Google Scholar

Murshudov, G. N., Skubak, P., Lebedev, A. A., Pannu, N. S., Steiner, R. A., Nicholls, R. A., et al. (2011). REFMAC5 for the refinement of macromolecular crystal structures. Acta Cryst. D 67, 355–367. doi: 10.1107/S0907444911001314

PubMed Abstract | CrossRef Full Text | Google Scholar

Nakada, Y., and Itoh, Y. (2003). Identification of the putrescine biosynthetic genes in Pseudomonas aeruginosa and characterization of agmatine deiminase and N-carbamoylputrescine amidohydrolase of the arginine decarboxylase pathway. Microbiology 149, 707–714. doi: 10.1099/mic.0.26009-0

PubMed Abstract | CrossRef Full Text | Google Scholar

Nakai, T., Hasegawa, T., Yamashita, E., Yamamoto, M., Kumasaka, T., Ueki, T., et al. (2000). Crystal structure of N-carbamyl-D-amino acid amidohydrolase with a novel catalytic framework common to amidohydrolases. Structure 8, 729–737. doi: 10.1016/S0969-2126(00)00160-X

PubMed Abstract | CrossRef Full Text | Google Scholar

Pace, H. C., and Brenner, C. (2001). The nitrilase superfamily: classification, structure and function. Genome Biol. 2, reviews0001.1–reviews0001.9. doi: 10.1186/gb-2001-2-1-reviews0001

CrossRef Full Text | Google Scholar

Penny, D. E., and Ritter, T. J. (1983). Kinetic-study of the reaction between carbon-dioxide and primary amines. J. Chem. Soci. Farad. Trans. I 79, 2103–2109. doi: 10.1039/F19837902103

CrossRef Full Text | Google Scholar

Pettersen, E. F., Goddard, T. D., Huang, C. C., Couch, G. S., Greenblatt, D. M., Meng, E. C., et al. (2004). UCSF Chimera–a visualization system for exploratory research and analysis. J. Comput. Chem. 25, 1605–1612. doi: 10.1002/jcc.20084

PubMed Abstract | CrossRef Full Text | Google Scholar

Piotrowski, M., Janowitz, T., and Kneifel, H. (2003). Plant C-N hydrolases and the identification of a plant N-carbamoylputrescine amidohydrolase involved in polyamine biosynthesis. J. Biol. Chem. 278, 1708–1712. doi: 10.1074/jbc.M205699200

PubMed Abstract | CrossRef Full Text | Google Scholar

Pottosin, I., and Shabala, S. (2014). Polyamines control of cation transport across plant membranes: implications for ion homeostasis and abiotic stress signaling. Front. Plant Sci. 5:154. doi: 10.3389/fpls.2014.00154

PubMed Abstract | CrossRef Full Text | Google Scholar

Pottosin, I., Velarde-Buendia, A. M., Bose, J., Fuglsang, A. T., and Shabala, S. (2014a). Polyamines cause plasma membrane depolarization, activate Ca2(-, and modulate H(-ATPase pump activity in pea roots. J. Exp. Bot. 65, 2463–2472. doi: 10.1093/jxb/eru133

PubMed Abstract | CrossRef Full Text | Google Scholar

Pottosin, I., Velarde-Buendia, A. M., Bose, J., Zepeda-Jazo, I., Shabala, S., and Dobrovinskaya, O. (2014b). Cross-talk between reactive oxygen species and polyamines in regulation of ion transport across the plasma membrane: implications for plant adaptive responses. J. Exp. Bot. 65, 1271–1283. doi: 10.1093/jxb/ert423

PubMed Abstract | CrossRef Full Text | Google Scholar

Puhl, A. A., Gruninger, R. J., Greiner, R., Janzen, T. W., Mosimann, S. C., and Selinger, L. B. (2007). Kinetic and structural analysis of a bacterial protein tyrosine phosphatase-like myo-inositol polyphosphatase. Protein Sci. 16, 1368–1378. doi: 10.1110/ps.062738307

PubMed Abstract | CrossRef Full Text | Google Scholar

Raczynska, J. E., Vorgias, C. E., Antranikian, G., and Rypniewski, W. (2011). Crystallographic analysis of a thermoactive nitrilase. J. Struct. Biol. 173, 294–302. doi: 10.1016/j.jsb.2010.11.017

PubMed Abstract | CrossRef Full Text | Google Scholar

Radhakrishnan, R., and Lee, I. J. (2013). Spermine promotes acclimation to osmotic stress by modifying antioxidant, abscisic acid, and jasmonic acid signals in soybean. J. Plant Growth Regul. 32, 22–30. doi: 10.1007/s00344-012-9274-8

CrossRef Full Text | Google Scholar

Roy, M., and Wu, R. (2001). Arginine decarboxylase transgene expression and analysis of environmental stress tolerance in transgenic rice. Plant Sci. 160, 869–875. doi: 10.1074/jbc.M205699200

PubMed Abstract | CrossRef Full Text | Google Scholar

Ruszkowski, M., Nocek, B., Forlani, G., and Dauter, Z. (2015). The structure of Medicago truncatula (1-pyrroline-5-carboxylate reductase provides new insights into regulation of proline biosynthesis in plants. Front. Plant Sci. 6:869. doi: 10.3389/fpls.2015.00869

PubMed Abstract | CrossRef Full Text | Google Scholar

Sakamoto, T., Sakata, S. F., Matsuda, K., Horikawa, Y., and Tamaki, N. (2001). Expression and properties of human liver beta-ureidopropionase. J. Nutr. Sci. Vitaminol. 47, 132–138. doi: 10.3177/jnsv.47.132

PubMed Abstract | CrossRef Full Text | Google Scholar

Sewell, B. T., Berman, M. N., Meyers, P. R., Jandhyala, D., and Benedik, M. J. (2003). The cyanide degrading nitrilase from Pseudomonas stutzeri AK61 is a two-fold symmetric, 14-subunit spiral. Structure 11, 1413–1422. doi: 10.1093/jxb/ert423

PubMed Abstract | CrossRef Full Text | Google Scholar

Shi, J., Fu, X. Z., Peng, T., Huang, X. S., Fan, Q. J., and Liu, J. H. (2010). Spermine pretreatment confers dehydration tolerance of citrus in vitro plants via modulation of antioxidative capacity and stomatal response. Tree Physiol. 30, 914–922. doi: 10.1093/treephys/tpq030

PubMed Abstract | CrossRef Full Text | Google Scholar

Shu, S., Yuan, L. Y., Guo, S. R., Sun, J., and Yuan, Y. H. (2013). Effects of exogenous spermine on chlorophyll fluorescence, antioxidant system and ultrastructure of chloroplasts in Cucumis sativus L. under salt stress. Plant Physiol. Biochem. 63, 209–216. doi: 10.1016/j.plaphy.2012.11.028

PubMed Abstract | CrossRef Full Text | Google Scholar

Tamaki, N., Mizutani, N., Kikugawa, M., Fujimoto, S., and Mizota, C. (1987). Purification and properties of beta-ureidopropionase from the rat liver. Eur. J. Biochem. 169, 21–26. doi: 10.1007/s00344-012-9274-8

CrossRef Full Text | Google Scholar

Terakado, J., Yoneyama, T., and Fujihara, S. (2006). Shoot-applied polyamines suppress nodule formation in soybean (Glycine max). J. Plant Physiol. 163, 497–505. doi: 10.1016/j.jplph.2005.05.007

PubMed Abstract | CrossRef Full Text | Google Scholar

Terwilliger, T. C., Grosse-Kunstleve, R. W., Afonine, P. V., Moriarty, N. W., Zwart, P. H., Hung, L. W., et al. (2008). Iterative model building, structure refinement and density modification with the PHENIX AutoBuild wizard. Acta Cryst. D 64, 61–69. doi: 10.1107/S090744490705024X

PubMed Abstract | CrossRef Full Text | Google Scholar

Thompson, J. D., Higgins, D. G., and Gibson, T. J. (1994). CLUSTAL W: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice. Nucleic Acids Res. 22, 4673–4680. doi: 10.1093/nar/22.22.4673

PubMed Abstract | CrossRef Full Text | Google Scholar

Thuku, R. N., Weber, B. W., Varsani, A., and Sewell, B. T. (2007). Post-translational cleavage of recombinantly expressed nitrilase from Rhodococcus rhodochrous J1 yields a stable, active helical form. FEBS J. 274, 2099–2108. doi: 10.1111/j.1742-4658.2007.05752.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Tiburcio, A. F., Altabella, T., Bitrian, M., and Alcazar, R. (2014). The roles of polyamines during the lifespan of plants: from development to stress. Planta 240, 1–18. doi: 10.1007/s00425-014-2055-9

PubMed Abstract | CrossRef Full Text | Google Scholar

Vassileva, V., and Ignatov, G. (1999). Polyamine-induced changes in symbiotic parameters of the Galega orientalis-Rhizobium galegae nitrogen-fixing system. Plant Soil 210, 83–91. doi: 10.1023/a:1004636800869

CrossRef Full Text | Google Scholar

Wang, B. Q., Zhang, Q. F., Liu, J. H., and Li, G. H. (2011). Overexpression of PtADC confers enhanced dehydration and drought tolerance in transgenic tobacco and tomato: effect on ROS elimination. Biochem. Biophys. Res. Commun. 413, 10–16. doi: 10.1016/j.bbrc.2011.08.015

PubMed Abstract | CrossRef Full Text | Google Scholar

Wang, W. C., Hsu, W. H., Chien, F. T., and Chen, C. Y. (2001). Crystal structure and site-directed mutagenesis studies of N-carbamoyl-D-amino-acid amidohydrolase from Agrobacterium radiobacter reveals a homotetramer and insight into a catalytic cleft. J. Mol. Biol. 306, 251–261. doi: 10.1006/jmbi.2000.4380

PubMed Abstract | CrossRef Full Text | Google Scholar

Winn, M. D., Ballard, C. C., Cowtan, K. D., Dodson, E. J., Emsley, P., Evans, P. R., et al. (2011). Overview of the CCP4 suite and current developments. Acta Cryst. D 67, 235–242. doi: 10.1107/S0907444910045749

PubMed Abstract | CrossRef Full Text | Google Scholar

Winn, M. D., Isupov, M. N., and Murshudov, G. N. (2001). Use of TLS parameters to model anisotropic displacements in macromolecular refinement. Acta Cryst. D 57, 122–133. doi: 10.1107/S0907444900014736

PubMed Abstract | CrossRef Full Text | Google Scholar

Winn, M. D., Murshudov, G. N., and Papiz, M. Z. (2003). Macromolecular TLS refinement in REFMAC at moderate resolutions. Methods Enzymol. 374, 300–321. doi: 10.1016/S0076-6879(03)74014-2

PubMed Abstract | CrossRef Full Text | Google Scholar

Xu, S. C., Hu, J., Li, Y. P., Ma, W. G., Zheng, Y. Y., and Zhu, S. J. (2011). Chilling tolerance in Nicotiana tabacum induced by seed priming with putrescine. Plant Growth Regul. 63, 279–290. doi: 10.1007/s10725-010-9528-z

CrossRef Full Text | Google Scholar

Yin, L., Wang, S., Tanaka, K., Fujihara, S., Itai, A., Den, X., and Zhang, S. (2016). Silicon-mediated changes in polyamines participate in silicon-induced salt tolerance in Sorghum bicolor L. Plant Cell Environ. 39, 245–258. doi: 10.1111/pce.12521

PubMed Abstract | CrossRef Full Text | Google Scholar

Zhang, Y., Zhang, H., Zou, Z. R., Liu, Y., and Hu, X. H. (2015). Deciphering the protective role of spermidine against saline-alkaline stress at physiological and proteomic levels in tomato. Phytochemistry 110, 13–21. doi: 10.1016/j.phytochem.2014.12.021

PubMed Abstract | CrossRef Full Text | Google Scholar

Keywords: polyamine synthesis, amidase mechanism, cadaverine, 1,4-diaminobutane, crystal structure, octamer, carbamoyl hydrolysis, CPA

Citation: Sekula B, Ruszkowski M, Malinska M and Dauter Z (2016) Structural Investigations of N-carbamoylputrescine Amidohydrolase from Medicago truncatula: Insights into the Ultimate Step of Putrescine Biosynthesis in Plants. Front. Plant Sci. 7:350. doi: 10.3389/fpls.2016.00350

Received: 23 December 2015; Accepted: 07 March 2016;
Published: 30 March 2016.

Edited by:

Patrick H. Masson, University of Wisconsin–Madison, USA

Reviewed by:

Carlos H. Ramos, University of Campinas, Brazil
Claude Alban, Institut National de la Recherche Agronomique, France

Copyright © 2016 Sekula, Ruszkowski, Malinska and Dauter. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.

*Correspondence: Milosz Ruszkowski, mruszkowski@anl.gov

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