Skip to main content

ORIGINAL RESEARCH article

Front. Plant Sci., 13 November 2017
Sec. Plant Physiology

Sulfated Polysaccharides in the Freshwater Green Macroalga Cladophora surera Not Linked to Salinity Adaptation

\r\nPaula X. ArataPaula X. Arata1Josefina AlberghinaJosefina Alberghina2Viviana ConfalonieriViviana Confalonieri2María I. ErreaMaría I. Errea3Jos M. Estevez*José M. Estevez4*Marina Ciancia,*Marina Ciancia1,5*
  • 1Universidad de Buenos Aires, Facultad de Agronomía, Departamento de Biología Aplicada y Alimentos, Cátedra de Química de Biomoléculas, Buenos Aires, Argentina
  • 2Universidad de Buenos Aires, Facultad de Ciencias Exactas y Naturales, Departamento de Ecología, Genética y Evolución, Instituto IEGEBA (UBA-CONICET), Buenos Aires, Argentina
  • 3Instituto Tecnológico de Buenos Aires, Departamento de Ingeniería Química, Buenos Aires, Argentina
  • 4Fundación Instituto Leloir-IIBBA-CONICET, Buenos Aires, Argentina
  • 5CONICET-Universidad de Buenos Aires, Centro de Investigación de Hidratos de Carbono (CIHIDECAR), Buenos Aires, Argentina

The presence of sulfated polysaccharides in cell walls of seaweeds is considered to be a consequence of the physiological adaptation to the high salinity of the marine environment. Recently, it was found that sulfated polysaccharides were present in certain freshwater Cladophora species and some vascular plants. Cladophora (Ulvophyceae, Chlorophyta) is one of the largest genera of green algae that are able to grow in both, seas and freshwater courses. Previous studies carried out on the water-soluble polysaccharides of the marine species C. falklandica established the presence of sulfated xylogalactoarabinans constituted by a backbone of 4-linked β-L-arabinopyranose units partially sulfated mainly on C3 and also on C2 with partial glycosylation, mostly on C2, with terminal β-D-xylopyranose or β-D-galactofuranose units. Besides, minor amounts of 3-, 6- and/or 3,6-linked β-D-galactan structures, with galactose in the pyranosic form were detected. In this work, the main water soluble cell wall polysaccharides from the freshwater alga Cladophora surera were characterized. It was found that this green alga biosynthesizes sulfated polysaccharides, with a structure similar to those found in marine species of this genus. Calibration of molecular clock with fossil data suggests that colonization of freshwater environments occurred during the Miocene by its ancestor. Therefore, the presence of sulfated polysaccharides in the freshwater green macroalga C. surera could be, in this case, an adaptation to transient desiccation and changes in ionic strength. Retention of sulfated polysaccharides at the cell walls may represent a snapshot of an evolutionary event, and, thus constitutes an excellent model for further studies on the mechanisms of sulfation on cell wall polysaccharides and environmental stress co-evolution.

Introduction

It has been proposed that the presence of sulfated polysaccharides in cell walls of seaweeds and marine angiosperms, absent in terrestrial plants, is a consequence of the physiological adaptation to the marine environment (Kloareg and Quatrano, 1988; Aquino et al., 2005) due to a strong environmental pressure. Most of sulfated polysaccharides present in seaweed (e.g., carrageenans) are well known to exhibit the solubility characteristics typical of hydrophilic colloids due to the presence of hydroxyl and sulfate groups in their backbones. Under certain conditions, they can form hydrogels, three-dimensional networks capable of maintaining a large amount of water. This moisture retention capacity is believed to be important for macroalgal desiccation resistance. Besides, their solubility characteristics are greatly affected by the salt form of their sulfate groups. Moreover, they show an important tendency to retain Ca2+and Mg2+, in agreement with their known capacity to retain these salts (Kloareg and Quatrano, 1988; Estevez et al., 2004). Sulfated polysaccharides produced by marine angiosperm Ruppia maritima Loisel disappeared when the plant was cultivated in the absence of salt (Aquino et al., 2011). On the other hand, the glycophyte Oryza sativa Linnaeus, when exposed to salt stress (200 mM NaCl) did not induce the biosynthesis of sulfated polysaccharides, but increased the concentration of carboxylated polysaccharides of the pectin type (Aquino et al., 2011). These data suggested that the presence of sulfated polysaccharides in marine plants is an adaptation to high-salinity environments, which may have been conserved during plant evolution from marine green algae (Aquino et al., 2011).

In an opposite way, very recently, it was found that, at least the green alga Cladophora glomerata and also Ulva flexuosa (Ulvophyceae, Chlorophyta), from two different freshwater environments (Nan river in Thailand and Lake Oporzynskie in Poland), with no detectable salt, were able to synthesize sulfated polysaccharides (Pankiewicz et al., 2016; Surayot et al., 2016). In both investigations, although the presence of sulfated polysaccharides was well established, the fine structures of polysaccharides where these sulfate groups were detected, were not conclusive, and further studies are required to confirm these findings. In addition, in the vascular plant Eichhornia crassipes, a native plant from Amazonas, also known as water hyacinth, collected in a freshwater tropical environment with no salinity, high quantities of sulfated polysaccharides were found in petioles, rhizome, and roots (Dantas-Santos et al., 2012). These highlighted examples suggest possible roles for cell wall sulfated polysaccharides in organisms exposed to stressful conditions different to salinity stress, like long periods of desiccation, high temperature exposure, transient changes in ionic strength in the water media (caused by water evaporation in small microsites), and so on.

The branched genus Cladophora (Ulvophyceae, Chlorophyta) is one of the largest genera of green algae that are able to grow in both, marine and fresh-water environments (Boedeker et al., 2016). We then decided to test if one species of Cladophora that grows in freshwater environments still retained the ability to modify its polysaccharides by the addition of sulfate groups, independently of the salinity stress. We chose to characterize the main cell wall components of C. surera E.R. Parodi and E.J. Cáceres due to the abundance of this freshwater alga in the southern part of Buenos Aires Province (Argentina) for at least 30 years (Parodi and Cáceres, 1991, 1995). Previous studies carried out on the water-soluble polysaccharides of several species of Cladophora from marine environments established the presence of sulfated xylogalactoarabinans (Percival and McDowell, 1981; Sri Ramana and Venkata Rao, 1991; Arata et al., 2016). Recently, the structure of the polysaccharides from C. falklandica was studied in detail, and it was found that they are constituted by a backbone of 4-linked β-L-arabinopyranose units partially sulfated mainly on C3 and also on C2 with partial glycosylation mostly on C2 with single β-D-xylopyranose, single β-D-galactofuranose units, or short β-D-galactofuranose chains comprising (1→5)- and/or (1→6)-linkages. Besides, minor amounts of 3-, 6- and 3,6-linked β-D-galactan structures, with galactose in the pyranosic form were detected.

Here, we have found that, although C. surera grows in a freshwater environment with no detected salt (as NaCl), it still biosynthesizes highly sulfated cell wall polymers. These results open new questions about the roles of sulfated polysaccharides, not necessarily linked to salt–stress, but possibly associated to a response to desiccation stress and changes in ionic strength of the environment in fluctuating freshwater habitats.

Materials and Methods

Algal Sample

Specimens of C. surera Parodi et Cáceres subsp. nov. were collected in Las Cascadas, Necochea, Buenos Aires Province (38°27′39′′ S 58°45′39′′ W) in April 2015 (Supplementary Figure S1). The water salinity at this site was < 1‰, measured with a Salinity Refractometer S/MIII, Cat No. 2441, ATAGO CO., LTD. Sulfate content of water at the collection site was determined by ion exchange chromatography with conductimetric detection using a DIONEX DX-100 chromatography system (Sunnyvale, CA, United States) with an AS4A column (4mm × 250 mm), an AMMS-II micromembrane suppressor; elution was carried out with 1.8 mM Na2CO3/1.7 mM NaHCO3, at a flow rate of 2 mL min-1.

Cladophora surera grew free floating in the freshwater course. Sporophytic and gametophytic plants are isomorphic. Measurements of length and width of cells from the principal axis and branches were within the range reported for this species by Parodi and Cáceres (1995). Gametangia developed from the upper cells in ultimate ramifications with similar dimensions and appearance to the vegetative cells. The samples used in this work were in the vegetative state. Thalli of the algae were washed with distilled water and analyzed for epiphytic and epizoic contaminants in a Nikon AFX-II macroscope (Nikon, Japan).

Phylogenetic Position of Cladophora surera

Genomic DNA was obtained from fresh algal material of C. surera using REDExtracts-N-Amp Tissue PCR Kit (SIGMA-ALDRICH). The nuclear-encoded small subunit (LSU) rDNA gene fragment was amplified and sequenced using primers and temperature profile as indicated in Boedeker and Immers (2009). Sequences were inspected and aligned using Geneious version 7.0 (Biomatters). SSU sequence was deposited in Gene Bank under accession number MF001434. The position of C. surera was investigated through the phylogenetic analyses of Thirty-two species of Cladophorales (Ulvophyceae), representing marine, brackish and freshwater environments (Accession numbers in Figure 1B). Two species from Ulvophyceae (U. curvata and Ulothrix zonata) were included as outgroups. Phylogenetic analyses of molecular characters were performed through Bayesian analysis (BA) as implemented in BEAST v1.6.2 (Drummond and Rambaut, 2007; Heled and Drummond, 2010). The model of sequence evolution was GTR+I+G (Rodríguez et al., 1990; Yang, 1994; Gu et al., 1995). Calibration of molecular clock was performed using the estimated minimum age of 600–570 million years for Cladophorales (van den Hoek and Chihara, 2000; Leliaert et al., 2007) based on fossil data. An uncorrelated relaxed clock model and a log-normal fossil calibration was used during tree searches. The number of Markov Chain Monte Carlo (MCMC) iterations was 30000000, from which the first 3000000 were discarded as non-converged burn-in; nodal support values were given as posterior probabilities.

FIGURE 1
www.frontiersin.org

FIGURE 1. Cell wall sulfated polysaccharides in the freshwater alga Cladophora surera. (A) General aspect of the alga. Scale bar = 5 cm. Branched filaments (Scale bar = 150 μm) and cell morphology with a well-developed cell wall (CW). Cyt = cytoplasm. Scale bar = 20 μm. (B) Bayesian tree, showing the phylogenetic position of C. surera collected in Quequén Grande river (Buenos Aires Province, Argentina). 1: Aegagropila clade; 2: Siphonocladus clade; 3: Cladophora clade. Scale-time bar underneath indicates million years. Left color bar indicates higher (red) to lower (green) posterior probabilities. Facultative or permanent fresh-water species. Arrowhead: putative events of freshwater colonization. Accession numbers are indicated with species names. (C) In situ distribution of sulfated polysaccharides, stained with TBO at pH7 (for anionic polysaccharides) and pH1 (for sulfated polysaccharides). Arrowheads indicate the presence of sulfated polysaccharides in two CW layers. Cyt = cytoplasm. Scale bar = 15 μm (top picture). Scale bar = 5 μm (bottom pictures). (D) Cross-sections of a C. surera cell after hot-water extraction (at 90°C) without staining (top panel) and stained with TBO at pH1 (bottom panel). Scale bar = 15 μm. (E) Attenuated Total Reflection-Fourier Transformed Infra-Red (ATR-FTIR) spectra of intact alga, of the hot-water CW extract (Cs90), and of the residue after exhaustive aqueous extraction (FR). Diagnostic bands for the presence of sulfate ester groups are highlighted at 1230 cm-1, due to asymmetric stretching of O = S = O and at 825 cm-1, due to stretching of Cecuatorial-O-S and/or Cprimary-O-S.

Light Microscopy and Histochemistry

For light microscopy (LM) semithin sections (10 μm) were mounted on glass slides and then observed with a Carl Zeiss Axiolab microscope (Carl Zeiss, Jena, Germany). The staining procedures used in LM histochemical characterization based on Krishnamurthy (1999), were carried out on the fixed tissues described above and included Toluidine Blue O (TBO; 0.05% w/v) in 0.1 m HCl at pH 1.0 that stains sulfated polysaccharides (red–purple, c metachromasia), and TBO at pH7 (for negatively charged polysaccharides). Hot water extraction at 90°C was carried out on cross-sections, which were then stained in conditions described above.

Extraction and Purification of the Polysaccharides

Algal samples of C. surera were dried in open air. The milled algae (100 g) were extracted twice with EtOH 70% (20g/L) for 3 h at room temperature. The residue from the alcohol extraction was extracted for 3 h with H2O (20 g/L) at 90°C, giving extract Cs90 (20.1 g). Cs90 was dissolved in water (4.5 mg/ml). A residue (Ri) was separated from the supernatant, which was chromatographed on DEAE-Sephadex A-25. The supernatant was applied to a column (90 cm × 1.5 cm id), previously stabilized in H2O. The first elution solvent was water and then NaCl solutions of increasing concentration up to 4 M. Fractions of 4 ml were collected. Finally, the phase was boiled in 4 M NaCl solution. The presence of carbohydrates in the samples was detected by the phenol sulfuric acid method (Dubois et al., 1956); after obtaining blank readings, the eluant was replaced by another with higher concentration of NaCl. Seven fractions (F1-F7) were obtained, dialyzed (molecular weight cut off 3,500) and freeze dried (Supplementary Figure S2).

Chemical Characterization

The total sugars content was analyzed by the phenol-sulfuric acid method (Dubois et al., 1956). Sulfate was determined turbidimetrically (Dodgson and Price, 1962). Alternatively, ion exchange chromatography with conductimetric detection was used: the sample was hydrolyzed in 2 M CF3COOH at 121°C for 2 h, evaporated to dryness under nitrogen and redissolved in high purity water from a Milli-Q system. A DIONEX DX-100 chromatography system (Sunnyvale, CA, United States) was used with an AS4A column (4 × 250 mm), an AMMS-II micromembrane suppressor and a conductivity detector, elution was carried out with 1.8 mM Na2CO3/1.7 mM NaHCO3, at a flow rate of 2 mL min-1. The absence of pyruvic acid and uronic acids was confirmed using the colorimetric determinations of Koepsell and Sharpe (1952) and Filisetti-Cozzi and Carpita (1991). The protein content was measured by microanalysis to determine the amount of nitrogen, a factor of 5 was applied to calculate the amount of protein, according to Angell et al. (2016). The configuration of galactose and arabinose was determined by the method of Cases et al. (1995) through their diastereomeric acetylated 1-deoxy-1-(2-hydroxypropylamino) alditols. To determine the monosaccharide composition, samples were derivatized to the alditol acetates (Stevenson and Furneaux, 1991).

Methylation Analysis

The sample (10–20 mg) was converted into the corresponding triethylammonium salt (Stevenson and Furneaux, 1991) and methylated according to Ciucanu and Kerek (1984). The sample was dissolved in dimethylsulfoxide; finely powdered NaOH was used as base. The methylated samples were submitted to reductive hydrolysis and acetylation to give the alditol acetates in the same way as the parent polysaccharides (Stevenson and Furneaux, 1991).

Gas Chromatography

GC of the alditol acetates were carried out on a Agilent 7890A gas-liquid chromatograph (Avondale, PA, United States) equipped with a flame ionization detector and fitted with a fused silica column (0.25mm i.d. × 30 m) WCOT-coated with a 0.20 mm film of SP-2330 (Supelco, Bellefonte, PA, United States). Chromatography was performed: from 200 to 240°C at 2°C min-1, followed by a 10-min hold for alditol acetates. For the partially methylated alditol acetates, the initial temperature was 160°C, which was increased at 1°C min-1 to 210°C and then at 2°C min-1 to 230°C. N2 was used as the carrier gas at a flow rate of 1 mL min-1 and the split ratio was 80:1. The injector and detector temperature was 250°C.

Gas Chromatography-Mass Spectrometry

GC–MS of the partially methylated alditol acetates was performed on a Agilent 7890A gas-liquid chromatograph equipped the SP-2330 interfaced to a Agilent 5977A Series mass spectrometer, working at 70 eV. The flow rate was 1.3 ml min-1, the injector temperature was 250°C. Mass spectra were recorded over a mass range of 30–500 amu.

Desulfation of Cs90

The reaction was carried out by the microwave-assisted method described by Navarro et al. (2007). The sample (40 mg) was converted to the pyridinium salt and dissolved in 10 ml of DMSO containing 2% of pyridine. The mixture was heated for 10 s intervals and cooled to 50°C (× 6). It was dyalized 3 days against tap water and then 24 h against distilled water (MWCO 3,500) and lyofilized. An aliquot was methylated as described above without previous isolation of the product.

Partial Acid Hydrolysis of Ri

The reaction was carried out according to Bilan et al. (2007). The sample (100 mg) was heated in 1% CH3COOH (20 mL) for 4 h at 100°C, the solution was neutralized with NaHCO3, dialyzed, and lyophilized to give RiH (78.2 mg). RiH was fractionated by anion exchange chromatography on DEAE-Sephadex A-25 in a similar way as F1, in this case, five fractions were obtained (RiH-F1-RiH-F5).

ATR-FTIR Spectroscopy

Samples were analyzed on a Thermo Scientific Nicolet 6700 spectrometer equipped with a smart ARK (Attenuated Reflectance Kit) accessory using a standard ZnSe crystal and a DTGS KBr detector. The spectra were recorded in the 650–4000 cm-1 range, and the spectral resolution was 4 cm-1. Data were processed by using the software Origin Pro 9.0.0.

NMR Spectroscopy

500 MHz 1H NMR, proton decoupled 125 MHz 13C NMR spectra, and two-dimensional NMR experiments (HSQC, HMBC, and COZY) were recorded on a Bruker AM500 at room temperature, with external reference of TMS. The samples (20 mg) were exchanged in 99.9% D2O (0.5 mL) four times. Chemical shifts were referenced to internal acetone (δH 2.175, δCH3 31.1). Parameters for 13C NMR spectra were as follows: pulse angle 51.4°, acquisition time 0.56 s, relaxation delay 0.6 s, spectral width 29.4 kHz, and scans 25,000. For 1H NMR spectra the parameters were: pulse angle 76°, acquisition time 3 s, relaxation delay 3 s, spectral width 6250 Hz and scans 32. 2D spectra were obtained using standard Bruker software.

Results and Discussion

Cladophora surera Biosynthesizes Sulfated Polysaccharides

Specimens of the green alga were collected in a freshwater environment (Quequén Grande river, 38°27′39′′ S 58°45′39′′ W) located in Buenos Aires Province, Argentina (Supplementary Figure S1). Based on the morphological characters, it was assigned to C. surera (Figure 1A; Parodi and Cáceres, 1991, 1995).

In order to gain further insight on the taxonomical identity, a molecular characterization of the SSU (nuclear-encoded small subunit rDNA) gene fragment of the collected species was carried out and its phylogenetic position within the Cladophorales was investigated. The Bayesian tree obtained (Figure 1B) recovered with high Posterior Probabilities (PP) the three major groups previously described by Boedeker et al. (2012): the “Aegagropila clade,” the “Siphonocladus clade” and the “Cladophora clade.” C. surera is resolved within the latter group, and particularly within a lineage of four species that can be mainly found in freshwater/brackish environments (Hanyuda et al., 2002; Boedeker et al., 2012). Within the order Cladophorales, the boundary between marine and freshwater environments was crossed at least two to three times (van den Hoek, 1963; Logares et al., 2007; Hayakawa et al., 2012; Boedeker et al., 2016; Figure 1B). Calibration of molecular clock with fossil data suggests that colonization of freshwater environments probably occurred 11.4 million years ago (MYA; 4–25 MYA 95% PP) by the ancestor of the four freshwater species closely related to C. surera (Figure 1B); or even before, at about 65.5 MYA (35–115 MYA 95%PP), during the diversification of the more basal species Rhizoclonium hieroglyphicum.

Cladophora surera showed a thick cell wall with two fibrillar-like layers delimiting a middle amorphous region. TBO staining suggested the presence of sulfated polysaccharides concentrated in both marginal cell wall layers (Figure 1C). Hot water extraction (at 90°C) carried out on cross-sections greatly suppressed TBO staining (Figure 1D). In agreement, the hot water extract (Cs90) obtained from C. surera that represents 20.1% (w/w) of the algal dry weight (Supplementary Figure S2) contained high amounts of sulfate (17%, as SO3Na, which correspond to ∼4% w/w of the algal dry weight), in accordance with the histochemical stainings.

Finally, Attenuated Total Reflection-Fourier Transformed Infra-Red (ATR-FTIR) spectrum of the dry milled alga, as well as that of extract Cs90 (Figure 1E) showed the bands diagnostic for the presence of sulfate ester groups at 1230 cm-1, which was assigned to asymmetric stretching of O = S = O, and at 825 cm-1, due to stretching of Cecuatorial-O-S and/or Cprimary-O-S (Prado Fernández et al., 2003). In agreement, after exhaustive sequential extraction with water (at 90°C) and with alkaline solutions, both IR bands (825 and 1230 cm-1) mostly disappeared in the remaining cell wall residue (FR) confirming that sulfated polysaccharides are confined in the aqueous extracts (Figure 1E).

All these results together confirmed the presence of high quantities of sulfated polysaccharides in cell walls of freshwater macroalga C. surera. The water salinity at the collection site was < 1‰ (w/w; as NaCl) and the sulfate content of the water was ∼1 mM, while usually in marine waters there are high sulfate concentrations (∼25–28 mM) (Bochenek et al., 2013). These results suggested that sulfated polysaccharides in some Cladophora species (at least in C. glomerata, and now in C. surera) could be synthetized in response to other stress factors, like desiccation and changes in ionic strength of the environment, not linked to high salinity levels as a stable environmental condition.

Sulfated Polysaccharides from Cladophora surera Have Common Structural Features with those of Marine Species of the Genus Cladophora

In order to characterize in depth the structure of these sulfated polysaccharides, with emphasis in the position of the sulfate groups on the carbohydrates backbone, the monosaccharide composition of the main cell wall extract obtained with hot water (Cs90) was determined. Cs90 is composed by arabinose and galactose as major monosaccharides, also important amounts of xylose were present (Table 1). Methylation analysis of Cs90 showed major quantities of 2,3-di-O-methyl-, 2-O-methyl-, 3-O-methyl-, and non-methylated arabinose, which correspond to 4-linked non-substituted, 3-substituted, 2-substituted, and disubstituted arabinose units (17, 28, 20, and 28 per 100 arabinose units, respectively) in the polysaccharide backbone. Desulfation of Cs90 gave Cs90D (Table 1), which by methylation analysis showed an important increase in 4-linked non-substituted arabinose units (A, ∼50% of the total arabinose units), and a decrease of 3-substituted (A3S) and 2,3-disubstituted units (A2,3S), while the percentage of 4-linked 2-substituted (A2X + A2R, R = chains up to four residues of Galp) units also increased to 38%. These results indicate that sulfate groups were mainly linked to C3 of the arabinopyranose units and in minor amounts, to C2 and C3, while some arabinose units were sulfated on C3 and substituted with single units of xylose or galactose on C2. Only minor amounts of galactofuranose units were detected. These units were previously found in important quantities in the arabinan of C. falklandica (Arata et al., 2016), and they were also detected in C. rupestris (Percival and McDowell, 1981, and references therein). Besides, methylation and desulfation–methylation analysis suggested the presence of short side chains of 3- and 3,6-linked galactopyranose units, partially sulfated on C4.

TABLE 1
www.frontiersin.org

TABLE 1. Yields and analyses of Cs90, the hot water extract from Cladophora surera, its desulfated derivative (Cs90D), and FiH3 a modified cell wall fraction.

As Cs90 had a limited solubility in water, it was not possible to carry out NMR spectroscopic analysis of this extract, however, good spectra were obtained from Cs90D (Figure 2A and Table 2), which allowed to determine that all the major monosaccharide units described above were in the β-configuration, and to confirm the linkages between them.

FIGURE 2
www.frontiersin.org

FIGURE 2. Average structure of sulfated xylogalactoarabinans, characterized by linkage analysis and Nuclear Magnetic Resonance (NMR) spectroscopy. 1H-13C Heteronuclear Single Quantum Coherence (HSQC) NMR spectra of (A) Cs90D and (B) FiH3 CW fractions. (C) Proposed structure of sulfated xylogalactoarabinan isolated from C. surera. Sulfated arabinose units are highlighted in red. Structural units: 4-linked β-L-arabinopyranose (A), 4-linked β-L-arabinopyranose sulfated at C-3 (A3S), 4-linked β-L-arabinopyranose disulfated at C2 and C3 (A2,3S), 4-linked β-L-arabinopyranose substituted with single units of β-D-xylopyranose at C2 (A2X), 4-linked β-L-arabinopyranose disubstituted with β-D-xylopyranose at C2 and sulfate at C3 (A2X3S), 4-linked β-L-arabinopyranose substituted at C2 with short chains up to four residues of β-L-galactopyranose (Gp; A2R) at C2. Non-reducing end A3S residues (nr) are also shown in the spectrum of FiH3.

TABLE 2
www.frontiersin.org

TABLE 2. Signal assignment of the HSQC NMR spectra of Cs90D and FiH3.

Besides, a strategy comprising controlled acid hydrolysis, fractionation by anion exchange chromatography (Supplementary Figure S2), and structural elucidation of the fractions by methylation analysis and NMR spectroscopy (Figures 2A,B and Table 2) was performed. Similar structural features were found in all the fractions obtained, but in different quantities. The highly purified sample FiH3 is shown as example (Figure 2B, and Tables 1, 2), and confirmed the structural features of these polysaccharides. As expected for FiH3, a fraction which eluted from an anion exchange chromatographic column with 2 M NaCl (Supplementary Figure S2), it is highly sulfated, and disulfated arabinose units are present in important amounts. In addition, it was found that in this fraction the β-D-galactopyranose units were mostly 6-linked and sulfated on C3. This structure was proposed based on methylation analysis, which showed the presence of 2,4-di-O-methylgalactose, as major partially methylated galactose derivative, and by the absence of a signal at δ 83.0/3.80 which would correspond to 3-linked β-D-galactopyranose units. Moreover, a small signal at δ 81.0/4.28 is a strong evidence for the presence of the mentioned 6-linked 3-sulfated galactose units. This substitution pattern of the galactan moiety was similar to that found in marine C. socialis (Sri Ramana and Venkata Rao, 1991). On the other hand, in C. falklandica, most of the galactose was in the furanosic form, and only minor quantities of 3-linked mostly 6-sulfated galactopyranose units were detected. Here, the important amount of terminal galactopyranose units, detected by methylation analysis and confirmed in the NMR spectra of Cs90D (Figure 2A and Table 2), indicates possible small side chains of up to ∼4 units of the arabinan backbone. These results suggest that the most important structural differences between the sulfated polysaccharides from species of Cladophora studied so far are restricted to the galactose units, while the pyranosic arabinan backbone and its sulfation pattern is conserved.

In conclusion, sulfated xylogalactoarabinans from cell walls of the freshwater alga C. surera have structural features similar to those reported for the marine species of this genus. Based on the structural determination carried out by linkage analysis and NMR spectroscopy, it is proposed that C. surera biosynthesizes sulfated xylogalactoarabinans as shown in Figure 2C.

Evolutionary Implications of the Presence of Sulfated Polysaccharides in C. surera

The presence of sulfated polysaccharides in C. surera is in agreement with two recent studies on C. glomerata from different freshwater environments (Nan river in Thailand and Lake Oporzynskie in Poland) (Pankiewicz et al., 2016; Surayot et al., 2016). In all three cases, they developed in freshwater environments. Sulfated polysaccharides are widespread in the cell walls of marine angiosperms, in marine algae (green, red, and brown seaweeds), in the extracellular matrix of vertebrate tissues, and in invertebrate species (Aquino et al., 2005; Ghandi and Mancera, 2008; Pomin and Mourao, 2008; Usov and Bilan, 2009; Ciancia et al., 2010; Usov, 2011). In the green alga Lamprothamnium papulosum (Characeae, Charophyta), which grows in water of fluctuating salinity, the extracellular sulfated mucilage increases in sulfate content with increasing salinity (Shepherd and Beilby, 1999; Shepherd et al., 1999), while in brown algae the concentrations of sulfate groups on fucans positively correlate with increasing exposure to the atmosphere in the intertidal zone, suggesting a role in desiccation resistance (Mabeau and Kloareg, 1987). Ectocarpus subulatus (Phaeophyta) isolated from a true freshwater environment (West and Kraft, 1996) undergoes major morphological, transcriptomic and metabolic changes under variable salinities, including alteration of the expression of genes encoding enzymes potentially involved in the sulfation or de-sulfation of cell wall polysaccharides (Dittami et al., 2012). It is now widely accepted that the occurrence of sulfated polysaccharides in phylogenetically distant taxa is a case of convergent adaptation to a broad range of environmental conditions, such as stable high ionic media (e.g., seawater for marine plants and algae) or transient changes in salt concentration linked to desiccation and high temperature stresses (e.g., in some cases of freshwater macroalgae and vascular plants) (Mabeau and Kloareg, 1987; Shepherd and Beilby, 1999; Shepherd et al., 1999; Aquino et al., 2011; Dantas-Santos et al., 2012; Pankiewicz et al., 2016; Surayot et al., 2016). From a physiological point of view, sulfated cell wall polysaccharides from marine plants and marine algae may confer an adaptive advantage through possible structural and osmotic functions that are linked to an environmental pressure. Terrestrialization, and the subsequent taxonomic proliferation of land plants, was predated by a divergence between the Chlorophyte (a group of green algae) and the Streptophyte lineages (which includes land plants). This is strongly correlated with a change in habitat preference from saline to freshwater conditions with low or no salt, as well as exposure to transient changes in ionic strength (e.g., caused by water evaporation in small microsites). These transitions are accompanied by a major alteration in cell wall polysaccharides composition such that, although the majority of marine Chlorophytes contain sulfated cell wall polysaccharides, they are largely absent from most of the freshwater Charophycean green algae and their descendants. The latter green algae contain large amounts of negatively charged pectins with carboxylated sugars (uronic acids) in their cell walls that could functionally replace some of the roles of sulfated polysaccharides (Domozych et al., 2012). Further studies to determine if sulfated polysaccharides are present in other freshwater algae are required to obtain a more comprehensive picture about their possible functions in the cell wall.

Conclusion

Although further evidence is required, early emerging freshwater and terrestrial organisms may have had a demand for sulfur that was in excess in the marine environment, but not in terrestrial and freshwater habitats (Raven, 1997). Such requirement for sulfate may have become a limiting factor and, therefore, may have been selected in organisms in a terrestrial environment, potentially resulting in the lack of carbohydrate sulfotransferases and sulfatases from the genomes of freshwater algae and land plants and sulfated polysaccharides from their cell walls (Popper et al., 2011). The case of both freshwater Cladophora species may indicate that not always the presence of sulfated polysaccharides provides an ionic barrier to high levels of salts, but it could be acting in response to other environmental factors like desiccation and transient changes in ionic strength media. It is important to note, that the effect of transient desiccation could give an important temporary increase in the ionic strength of the medium. Also, the high temperatures, in which plants in tropical regions develop, could cause desiccation. So, all these factors could be linked to high ionic strength environments, permanent or lasting only a short period of time. Hence, retention of sulfation capacity in freshwater Cladophora species could be due to this factor, as well as to water retention capacity. Colonization of freshwater environments by the ancestor of the four freshwater Cladophora species closely related to C. surera probably occurred during the Miocene. Retention of sulfated polysaccharides at the cell walls of freshwater green macroalgae may represent a more general phenomenon, which constitutes an excellent model for further studies on the mechanisms of sulfation on cell wall polysaccharides and stress factors in freshwater environments co-evolution. Further genomic and physiological studies are required to understand the molecular basis of the retention of sulfated polysaccharides in C. surera in a freshwater environment. Finally, it is tempting to suggest for future studies that sulfated polysaccharides could have, in this case, unknown masked functions, not related to salinity adaptation.

Author Contributions

PA, JA, and ME performed the experiments, VC analyzed and discussed the phylogenetic data, MC programmed the experiments, JE and MC dicussed the results and wrote the manuscript.

Funding

This work was supported by a grant from the University of Buenos Aires (UBACYT 2014-2017, 20020130100576BA) and Ministerio de Ciencia, Tecnología e Innovación Productiva (PICT2014-0504).

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.

The reviewer KM and handling Editor declared their shared affiliation.

Acknowledgments

VC, JE, and MC are Research Member of the National Research Council of Argentina (CONICET). Authors are indebted to Juan Pablo Basualdo for technical support.

Supplementary Material

The Supplementary Material for this article can be found online at: https://www.frontiersin.org/articles/10.3389/fpls.2017.01927/full#supplementary-material

FIGURE S1 | Maps showing the collecting site of the green macroalgae Cladophora surera located in Buenos Aires Province, Argentina (A). Specimens of a green macroalgae were collected in a fresh-water environment of Quequén Grande river (38°27′39′′ S 58°45′39′′ W) (B).

References

Angell, A. R., Mata, L., de Nys, R., and Paul, N. A. (2016). The protein content of seaweeds: a universal nitrogen-to-protein conversion factor of five. J. Appl. Phycol. 28, 511–524. doi: 10.1007/s10811-015-0650-1

CrossRef Full Text | Google Scholar

Aquino, R. S., Grativol, C., and Mourão, P. A. S. (2011). Rising from the sea: correlations between sulfated polysaccharides and salinity in plants. PLOS ONE 6:e18862. doi: 10.1371/journal.pone.0018862

PubMed Abstract | CrossRef Full Text | Google Scholar

Aquino, R. S., Landeira-Fernandez, A. M., Valente, A. P., Andrade, L. R., and Mourao, P. A. (2005). Occurrence of sulfated galactans in marine angiosperms: evolutionary implications. Glycobiology 15, 11–20. doi: 10.1093/glycob/cwh138

PubMed Abstract | CrossRef Full Text | Google Scholar

Arata, P. X., Quintana, I., Raffo, M. P., and Ciancia, M. (2016). Novel sulfated xylogalactoarabinans from green seaweed Cladophora falklandica: chemical structure and action on the fibrin network. Carbohydr. Polym. 154, 139–150. doi: 10.1016/j.carbpol.2016.07.088

PubMed Abstract | CrossRef Full Text | Google Scholar

Bilan, M. I., Vinogradova, E. V., Shashkov, A. S., and Usov, A. I. (2007). Structure of a highly pyruvylated galactan sulfate from the pacific green alga Codium yezoense (Bryopsidales, Chlorophyta). Carbohydr. Res. 342, 586–596. doi: 10.1016/j.carres.2006.11.008

PubMed Abstract | CrossRef Full Text | Google Scholar

Bochenek, M., Etherington, G. J., Koprivova, A., Mugford, S. T., Bell, T. G., Malin, G., et al. (2013). Transcriptome analysis of the sulfate deficiency response in the marine microalga Emiliania huxleyi. New Phytol. 199, 650–662. doi: 10.1111/nph.12303

PubMed Abstract | CrossRef Full Text | Google Scholar

Boedeker, C., and Immers, A. (2009). No more lake balls (Aegagropila linnaei Kützing, Cladophoraphyceae, Chlorophyta) in the Netherlands? Aquat. Ecol. 43, 891–902. doi: 10.1007/s10452-009-9231-1

CrossRef Full Text | Google Scholar

Boedeker, C., Leliaert, F., and Zuccarello, G. C. (2016). Molecular phylogeny of the Cladophoraceae (Cladophorales, Ulvophyceae), with the resurrection of Acrocladus Nägeli and Willeella Børgesen, and the description of Lubrica gen. nov. and Pseudorhizoclonium gen. nov. J. Phycol. 52, 905–928. doi: 10.1111/jpy.12457

PubMed Abstract | CrossRef Full Text | Google Scholar

Boedeker, C., O’Kelly, C. J., Star, W., and Leliaert, F. (2012). Molecular phylogeny and taxonomy of the Aegagropila clade (Cladophorales, Chlorophyta), including the description of Aegagropilopsis gen. nov. and Pseudocladophora gen. nov. J. Phycol. 48, 808–825. doi: 10.1078/1434-4610-00068

PubMed Abstract | CrossRef Full Text | Google Scholar

Cases, M. R., Cerezo, A. S., and Stortz, C. A. (1995). Separation and quantitation of enantiomeric galactoses and their mono-O-methylethers as their diastereomeric acetylated 1-deoxy-1-(2-hydroxypropylamino) alditols. Carbohydr. Res. 269, 333–341. doi: 10.1016/0008-6215(94)00370-U

CrossRef Full Text | Google Scholar

Ciancia, M., Quintana, I., and Cerezo, A. S. (2010). Overview of anticoagulant activity of sulfated polysaccharides from seaweeds in relation to their structures, focusing on those of green seaweeds. Curr. Med. Chem. 17, 2503–2529. doi: 10.2174/092986710791556069

PubMed Abstract | CrossRef Full Text | Google Scholar

Ciucanu, I., and Kerek, K. (1984). A simple and rapid method for the permethylation of carbohydrates. Carbohydr. Res. 134, 209–217. doi: 10.1016/0008-6215(84)85242-8

CrossRef Full Text | Google Scholar

Dantas-Santos, N., Gomes, D. L., Costa, L. S., Cordeiro, S. L., Costa, M. S., Trindade, E. S., et al. (2012). Freshwater plants synthesize sulfated polysaccharides: heterogalactans from water hyacinth (Eicchornia crassipes). Int. J. Mol. Sci. 13, 961–976. doi: 10.3390/ijms13010961

PubMed Abstract | CrossRef Full Text | Google Scholar

Dittami, S. M., Gravot, A., Goulitquer, S., Rousvoal, S., Peters, A. F., Bouchereau, A., et al. (2012). Towards deciphering dynamic changes and evolutionary mechanisms involved in the adaptation to low salinities in Ectocarpus (brown algae). Plant J. 71, 366–377. doi: 10.1111/j.1365-313X.2012.04982.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Dodgson, K. S., and Price, R. G. (1962). A note on the determination of the ester sulphate content of sulphated polysaccharides. Biochem. J. 84, 106–110. PMCID: PMC1243628 doi: 10.1042/bj0840106

PubMed Abstract | CrossRef Full Text | Google Scholar

Domozych, D. S., Ciancia, M., Fangel, J., Mikkelsen, M. D., Ulvskov, P., and Willats, W. G. T. (2012). The cell walls of green algae: a journey through evolution and diversity. Front. Plant Sci. 3:82. doi: 10.3389/fpls.2012.00082

PubMed Abstract | CrossRef Full Text

Drummond, A. J., and Rambaut, A. (2007). Beast: Bayesian evolutionary analysis by sampling trees. BMC Evol. Biol. 7:214. doi: 10.1186/1471-2148-7-214

PubMed Abstract | CrossRef Full Text | Google Scholar

Dubois, M., Gilles, K. A., Hamilton, J. K., Rebers, P. A., and Smith, F. (1956). Colorimetric method of determination of sugars and related substances. Anal. Chem. 28, 350–356. doi: 10.1021/ac60111a017

PubMed Abstract | CrossRef Full Text | Google Scholar

Estevez, J. M., Ciancia, M., and Cerezo, A. S. (2004). The system of galactans of the red seaweed, Kappaphycus alvarezii, with emphasis on its minor constituents. Carbohydr. Res. 339, 2575–2592. doi: 10.1016/j.carres.2004.08.010

PubMed Abstract | CrossRef Full Text | Google Scholar

Filisetti-Cozzi, T. M., and Carpita, N. C. (1991). Measurement of uronic acids without interference from neutral sugars. Anal. Biochem. 197, 157–162. doi: 10.1016/0003-2697(91)90372-Z

PubMed Abstract | CrossRef Full Text | Google Scholar

Ghandi, N. S., and Mancera, R. L. (2008). The structure of glycosaminoglycans and their interactions with proteins. Chem. Biol. Drug Des. 72, 455–482. doi: 10.1111/j.1747-0285.2008.00741.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Gu, X., Fu, Y. X., and Li, W. H. (1995). Maximum likelihood estimation of the heterogeneity of substitution rate among nucleotide sites. Mol. Biol. Evol. 12, 546–557. doi: 10.1093/oxfordjournals.molbev.a040235

CrossRef Full Text | Google Scholar

Hanyuda, T., Wakana, I., Arai, S., Miyaj, I. K., Watano, Y., and Ueda, K. (2002). Phylogenetic relationships between Cladophorales (Ulvophyceae, Chlorophyta) inferred from 18S rRNA gene sequences, with special reference to Aegagropila linnei. J. Phycol 38, 564–571. doi: 10.1046/j.1529-8817.2002.01151.x

CrossRef Full Text | Google Scholar

Hayakawa, Y. I., Ogawa, T., Yoshikawa, S., Ohki, K., and Kamiya, M. (2012). Genetic and ecophysiological diversity of Cladophora (Cladophorales, Ulvophyceae) in various salinity regimes. Phycol. Res. 60, 86–97. doi: 10.1111/j.1440-1835.2012.00641.x

CrossRef Full Text | Google Scholar

Heled, J., and Drummond, A. J. (2010). Bayesian inference of species trees from multilocus data. Mol. Biol. Evol. 27, 570–580. doi: 10.1093/molbev/msp274

PubMed Abstract | CrossRef Full Text | Google Scholar

Kloareg, B., and Quatrano, R. S. (1988). Structure of the cell wall of marine algae and ecophysiological functions of the matrix polysaccharides. Oceanogr. Mar. Biol. Annu. Rev. 26, 259–315.

Google Scholar

Koepsell, H. J., and Sharpe, E. S. (1952). Microdetermination of pyruvic and α-ketoglutaric acids. Arch. Biochem. Biophys. 38, 443–449. doi: 10.1016/0003-9861(52)90050-7

PubMed Abstract | CrossRef Full Text | Google Scholar

Krishnamurthy, K. V. (1999). “Transmission electron microscopic cytochemistry,” in Methods in Cell Wall Cytochemistry, ed. K. V. Krishnamurthy (Boca Raton, FL: CRC Press), 177–226.

Google Scholar

Leliaert, F., De Clerck, O., Verbruggen, H., Boedeker, C., and Coppejans, E. (2007). Molecular phylogeny of the Siphonocladales (Chlorophyta: Cladophorophyceae). Mol. Phylogenet. Evol. 44, 1237–1256. doi: 10.1016/j.ympev.2007.04.016

PubMed Abstract | CrossRef Full Text | Google Scholar

Logares, R., Shalchian-Tabrizi, K., Boltovskoy, A., and Rengefors, K. (2007). Extensive dinoflagellate phylogenies indicate infrequent marine–freshwater transitions. Mol. Phylogen. Evol. 45, 887–903. doi: 10.1016/j.ympev.2007.08.005

PubMed Abstract | CrossRef Full Text | Google Scholar

Mabeau, S., and Kloareg, B. (1987). Isolation and analysis of the cell walls of brown algae: Fucus spiralis, F. ceranoides, F. vesiculosus, F. serratus, Bifurcaria bifurcata and Laminaria digitata. J. Exp. Bot. 38, 1573–1580. doi: 10.1093/jxb/38.9.1573

CrossRef Full Text | Google Scholar

Navarro, D. A., Flores, M. L., and Stortz, C. A. (2007). Microwave-assisted desulfation of sulfated polysaccharides. Carbohydr. Polym. 69, 742–747. doi: 10.1016/j.carbpol.2007.02.009

CrossRef Full Text | Google Scholar

Pankiewicz, R., Ł˛eska, B., Messyasz, L., Fabrowska, J., Sołoducha, M., and Pikosz, M. (2016). First isolation of polysaccharidic ulvans from the cell walls of freshwater algae. Algal Res. 19, 348–354. doi: 10.1016/j.algal.2016.02.025

CrossRef Full Text | Google Scholar

Parodi, E. R., and Cáceres, E. J. (1991). Variation in number of apical ramifications and vegetative cell length in freshwater populations of Cladophora (Ulvophyceae, Chlorophyta). J. Phycol. 27, 628–633. doi: 10.1111/j.0022-3646.1991.00628.x

CrossRef Full Text | Google Scholar

Parodi, E. R., and Cáceres, E. J. (1995). Life history of Cladophora surera sp. Nov. (Cladophorales, Ulvophyceae). Phycol. Res. 43, 223–231. doi: 10.1111/j.1440-1835.1995.tb00028.x

CrossRef Full Text | Google Scholar

Percival, E., and McDowell, R. H. (1981). “Algal walls: composition and biosynthesis,” in Encyclopedia of Plant Physiology, Vol. 13B, eds W. Tanner and F. A. Loewus (Berlin: Springer), 277–316.

Google Scholar

Pomin, V. H., and Mourao, P. A. (2008). Structure, biology, evolution, and medical importance of sulfated fucans and galactans. Glycobiology 18, 1016–1027. doi: 10.1093/glycob/cwn085

PubMed Abstract | CrossRef Full Text | Google Scholar

Popper, Z. A., Michel, G., Hervé, C., Domozych, D. S., Willats, W. G. T., Tuohy, M. G., et al. (2011). Evolution and diversity of plant cell walls: from algae to flowering plants. Annu. Rev. Plant Biol. 62, 567–590. doi: 10.1146/annurev-arplant-042110-103809

PubMed Abstract | CrossRef Full Text | Google Scholar

Prado Fernández, J., Rodríguez Vazquez, J. A., Tojo, E., and Andrade, J. M. (2003). Quantitation of κ-, ι- and λ-carrageenan by midinfrared spectroscopy and PLS regression. Anal. Chim. Acta 480, 23–37. doi: 10.1016/S0003-2670(02)01592-1

CrossRef Full Text | Google Scholar

Raven, J. A. (1997). The role of marine biota in the evolution of terrestrial biota: gases and genes. Biogeochemistry 39, 139–164. doi: 10.1023/A:1005855528289

CrossRef Full Text | Google Scholar

Rodríguez, F., Oliver, J. L., Marín, A., and Medina, J. R. (1990). The general stochastic model of nucleotide substitution. J. Theor. Biol. 142, 485–501. doi: 10.1016/S0022-5193(05)80104-3

CrossRef Full Text | Google Scholar

Shepherd, V. A., and Beilby, M. J. (1999). The effect of an extracellular mucilage on the response to osmotic shock in the charophyte alga Lamprothamnium papulosum. J. Membr. Biol. 170, 229–242. doi: 10.1007/s002329900552

PubMed Abstract | CrossRef Full Text | Google Scholar

Shepherd, V. A., Beilby, M. J., and Heslop, D. J. (1999). Ecophysiology of the hypotonic response in the salt-tolerant charophyte alga Lamprothamnium papulosum. Plant Cell Environ. 22, 333–346. doi: 10.1046/j.1365-3040.1999.00414.x

CrossRef Full Text | Google Scholar

Sri Ramana, K., and Venkata Rao, E. (1991). Structural features of the sulphated polysaccharide from a green seaweed, Cladophora socialis. Phytochemistry 30, 259–262. doi: 10.1016/0031-9422(91)84133-D

PubMed Abstract | CrossRef Full Text | Google Scholar

Stevenson, T. T., and Furneaux, R. H. (1991). Chemical methods for the analysis of sulphated galactans from red algae. Carbohydr. Res. 210, 277–298. doi: 10.1016/0008-6215(91)80129-B

PubMed Abstract | CrossRef Full Text | Google Scholar

Surayot, U., Lee, J. H., Kanongnuch, C., Peerapornpisal, Y., Park, W. J., and You, S. G. (2016). Structural characterization of sulfated arabinans extracted from Cladophora glomerata Kützing and their macrophage activation. Biosci. Biotechnol. Biochem. 80, 972–982. doi: 10.1080/09168451.2015.1132149

PubMed Abstract | CrossRef Full Text | Google Scholar

Usov, A. I. (2011). Polysaccharides of the red algae. Adv. Carbohydr. Chem. Biochem. 65, 115–217. doi: 10.1016/B978-0-12-385520-6.00004-2

PubMed Abstract | CrossRef Full Text | Google Scholar

Usov, A. I., and Bilan, M. I. (2009). Fucoidans-sulfated polysaccharides of brown algae. Russ. Chem. Rev. 78, 785–799. doi: 10.1070/RC2009v078n08ABEH004063

CrossRef Full Text | Google Scholar

van den Hoek, C. (1963). Revision of the European Species of Cladophora. Leiden: Brill Archive, 248.

Google Scholar

van den Hoek, C., and Chihara, M. (2000). A taxonomic revision of the marine species of Cladophora (Chlorophyta) along the coasts of Japan and the Russian Far-east. Nat. Sci. Mus. Monogr. 19, 242.

Google Scholar

West, J., and Kraft, G. (1996). Ectocarpus siliculosus (Dillwyn) Lyngb. from hopkins river falls, victoria-the first record of a freshwater brown alga in Australia. Muelleria 9, 29–33.

Google Scholar

Yang, Z. (1994). Maximum likelihood phylogenetic estimation from DNA sequences with variable rates over sites: approximate methods. J. Mol. Evol. 39, 306–314. doi: 10.1007/BF00160154

PubMed Abstract | CrossRef Full Text | Google Scholar

Keywords: green alga, Cladophora, cell walls, sulfated polysaccharides, freshwater environment

Citation: Arata PX, Alberghina J, Confalonieri V, Errea MI, Estevez JM and Ciancia M (2017) Sulfated Polysaccharides in the Freshwater Green Macroalga Cladophora surera Not Linked to Salinity Adaptation. Front. Plant Sci. 8:1927. doi: 10.3389/fpls.2017.01927

Received: 16 August 2017; Accepted: 25 October 2017;
Published: 13 November 2017.

Edited by:

Wim Van den Ende, KU Leuven, Belgium

Reviewed by:

Koenraad Muylaert, KU Leuven, Belgium
Céline Laroche, Université Clermont Auvergne, France

Copyright © 2017 Arata, Alberghina, Confalonieri, Errea, Estevez and Ciancia. 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: Marina Ciancia, ciancia@agro.uba.ar José M. Estevez, jestevez@leloir.org.ar

Disclaimer: All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article or claim that may be made by its manufacturer is not guaranteed or endorsed by the publisher.