Marta Derba-Maceluch1
Pramod Sivan1,2
Evgeniy N. Donev1
Madhavi Latha Gandla3
Zakiya Yassin4
Rakhesh Vaasan2Emilia Heinonen2,5Sanna Andersson1Fariba Amini6,7Gerhard Scheepers4Ulf Johansson8
Francisco J. Vilaplana2,5
Benedicte R. Albrectsen6Magnus Hertzberg9
Leif J. Jönsson3
Ewa J. Mellerowicz1*- 1Umeå Plant Science Centre, Department of Forest Genetics and Plant Physiology, Swedish University of Agricultural Sciences, Umeå, Sweden
- 2Division of Glycoscience, Department of Chemistry, KTH Royal Institute of Technology, AlbaNova University Centre, Stockholm, Sweden
- 3Department of Chemistry, Umeå University, Umeå, Sweden
- 4Enhet Produktionssystem och Material, RISE Research Institutes of Sweden, Växjö, Sweden
- 5Wallenberg Wood Science Centre (WWSC), KTH Royal Institute of Technology, Stockholm, Sweden
- 6Umeå Plant Science Centre, Department of Plant Physiology, Umeå University, Umea, Sweden
- 7Biology Department, Faculty of Science, Arak University, Arak, Iran
- 8Tönnersjöheden Experimental Forest, Swedish University of Agricultural Sciences, Simlångsdalen, Sweden
- 9SweTree Technologies AB, Umeå, Sweden
Xylan that comprises roughly 25% of hardwood biomass is undesirable in biorefinery applications involving saccharification and fermentation. Efforts to reduce xylan levels have therefore been made in many species, usually resulting in improved saccharification. However, such modified plants have not yet been tested under field conditions. Here we evaluate the field performance of transgenic hybrid aspen lines with reduced xylan levels and assess their usefulness as short-rotation feedstocks for biorefineries. Three types of transgenic lines were tested in four-year field tests with RNAi constructs targeting either Populus GT43 clades B and C (GT43BC) corresponding to Arabidopsis clades IRX9 and IRX14, respectively, involved in xylan backbone biosynthesis, GATL1.1 corresponding to AtGALT1 involved in xylan reducing end sequence biosynthesis, or ASPR1 encoding an atypical aspartate protease. Their productivity, wood quality traits, and saccharification efficiency were analyzed. The only lines differing significantly from the wild type with respect to growth and biotic stress resistance were the ASPR1 lines, whose stems were roughly 10% shorter and narrower and leaves showed increased arthropod damage. GT43BC lines exhibited no growth advantage in the field despite their superior growth in greenhouse experiments. Wood from the ASPR1 and GT43BC lines had slightly reduced density due to thinner cell walls and, in the case of ASPR1, larger cell diameters. The xylan was less extractable by alkali but more hydrolysable by acid, had increased glucuronosylation, and its content was reduced in all three types of transgenic lines. The hemicellulose size distribution in the GALT1.1 and ASPR1 lines was skewed towards higher molecular mass compared to the wild type. These results provide experimental evidence that GATL1.1 functions in xylan biosynthesis and suggest that ASPR1 may regulate this process. In saccharification without pretreatment, lines of all three constructs provided 8-11% higher average glucose yields than wild-type plants. In saccharification with acid pretreatment, the GT43BC construct provided a 10% yield increase on average. The best transgenic lines of each construct are thus predicted to modestly outperform the wild type in terms of glucose yields per hectare. The field evaluation of transgenic xylan-reduced aspen represents an important step towards more productive feedstocks for biorefineries.
1 Introduction
Lignocellulose derived from plant cell walls is the largest source of carbon on the Earth (Bar-On et al., 2018) and can be used for sustainable production of energy carriers, green chemicals, and materials. Xylan constitutes approx. 20-30% of lignocellulose in hardwoods, 40-50% in grasses, and 5-15% in softwoods (Scheller and Ulvskov, 2010). It is usually seen as a negative factor in saccharification and fermentation processes because it restricts access to cellulose, cross-links lignin, and forms xylose when hydrolyzed, which is undesirable because xylose is used inefficiently by ethanol-producing yeasts (Donev et al., 2018; Wierzbicki et al., 2019). Xylan in hardwoods and grasses is also an important source of acetic acid in saccharification/fermentation media which is one of the main inhibitors of alcoholic fermentation with yeast (Jönsson and Martín, 2016). Efforts to reduce the xylan content of the lignocellulose or change its structure have therefore been made in many species by suppressing various xylan biosynthetic genes. These measures usually have positive effects on saccharification but may also adversely affect growth (reviewed by Donev et al., 2018, and Wierzbicki et al., 2019). Fortunately, these negative effects can often be avoided or even reversed by fine tuning the degree of gene suppression (Biswal et al., 2015; Ratke et al., 2018). However, field tests of improved xylan-modified plants have only been reported for hybrid aspen (Populus tremula L. x tremuloides Michx.) lines with reduced xylan acetylation (Derba-Maceluch et al., 2020; Pramod et al., 2021). Other types of xylan modification have only been tested under greenhouse conditions.
A genetic engineering strategy for xylan reduction in aspen that has performed especially well in greenhouse experiments involves suppressing genes of clades B and C in the GT43 family, corresponding to Arabidopsis clades IRX9 and IRX14, respectively, which encode proteins belonging to the secondary wall xylan synthase complex (Ratke et al., 2015). These genes are required for the proper function of the xylan UDP-xylosyl transferase complex in Arabidopsis, Populus and other plant species (Brown et al., 2007; Lee et al., 2007a; Zhou et al., 2007; Lee et al., 2010; Lee et al., 2011; Lee et al., 2012; Ratke et al., 2018). The proteins of these two clades bind the xylan xylosyl transferase encoded by a GT47 member IRX10 (Jensen et al., 2014; Jiang et al., 2016; Zeng et al., 2016) and are essential for both assembly of the complex in the ER and Golgi and its subsequent anchoring to the membrane (Anders et al., 2023). Suppressing these genes in hybrid aspen improved growth and enzymatic saccharification yields (Ratke et al., 2018) and could thus partially alleviate the need for chemical pretreatment of biorefinery feedstocks. However, practical deployment of such modified feedstocks will require field testing of the modified lines.
The biosynthesis of the xylan backbone in dicotyledons and conifers requires the synthesis of a tetrasaccharide known as the reducing-end sequence (RES) that is bound to the backbone at the reducing end (Peña et al., 2007). Mutations in genes responsible for RES biosynthesis reduce xylan levels and secondary wall thickness, producing a so-called “irregular xylem” (irx) phenotype resembling that of xylan synthase mutants (Brown et al., 2007; Peña et al., 2007; Lee et al., 2007b; Brown et al., 2009). At least three genes are known to participate in RES biosynthesis in Arabidopsis: GAUT12/IRX8, GATL1/PARVUS and FRA8/IRX7 (reviewed by Smith et al., 2018). Populus has either one or two copies of each of these genes: the copies of AtGAUT12 are GAUT12-1 and GAUT12-2, which are also known as GT8D1/GAUT12-A and GT8D2/GAUT12-B (Li et al., 2011; Biswal et al., 2015; Kumar et al., 2019); the copies of AtGATL1 are GATL1.1 and GATL1.2, also known as GT8E/GATL1-A and GT8F/GATL1-B (Kong et al., 2009; Lee et al., 2009a; Kumar et al., 2019); and the copy of AtFRA8 is GT47C (Zhou et al., 2006). These Populus genes complement the corresponding Arabidopsis mutants (Zhou et al., 2006; Kong et al., 2009; Lee et al., 2009a; Biswal et al., 2015) and are thus predicted to function in RES biosynthesis. Suppression of GAUT12-1 and GT47C in Populus resulted in decreased xylan content, thinner secondary walls, improved saccharification, and in the case of GAUT12-1 also in increased growth (Lee et al., 2009b; Lee et al., 2011; Li et al., 2011; Biswal et al., 2015), whereas simultaneous suppression of GAUT12-1 and GAUT12-2 induced lignification and brittle stems in greenhouse-grown trees (Li et al., 2011). The effects of suppressing GATL1.1 and GATL1.2 have not been analyzed to date. Other genes that may participate in xylan backbone biosynthesis include IRX15 in Arabidopsis (Jensen et al., 2011) and genes encoding a germin-like protein and VERNALIZATION PROTEIN 2 in wheat (Jiang et al., 2016). However, the biochemical functions of these genes are currently unknown. Additionally, no xylan backbone or RES sequence biosynthetic mutants or knock-down (KD) lines have been tested under field conditions.
Here we evaluate the field phenotypes of transgenic hybrid aspen lines with suppressed expression of the B and C clades of GT43 family genes and GATL1.1 based on a four-year field experiment in Southern Sweden. We also report a novel xylan defect in aspen lines with suppressed expression of ASPARTIC PROTEASE 1 (ASPR1) which was not previously implicated in xylan biosynthesis but was tested here since the gene was highly induced during secondary wall formation in developing wood (Sundell et al., 2017). We evaluate these three genetic modifications in terms of field productivity and biomass saccharification potential to determine their usefulness in efforts to engineer short-rotation biorefinery feedstocks.
2 Materials and methods
2.1 Plant material
Hybrid aspen (Populus tremula L. x tremuloides Michx.) clone T89 was used to make transgenic lines (Table 1) and as a wild-type (WT) control. Vectors for generation of 35S:ASPR1 and 35S:GATL1.1 lines were based on the plant RNAi vector pK7GWIWG2; cloned cDNA fragments (Table S1) were inserted between the vector’s attR1 and attR2 using the GATEWAY system (Karimi et al., 2002). The generation of WP : GT43BC lines was described in an earlier publication (Ratke et al., 2018). Transgenic lines were obtained by Agrobacterium transformation and clonally replicated in vitro as described previously (Ratke et al., 2018). The lines used in the experiment were chosen from 10-20 independent clones based on transgene expression and phenotypes in greenhouse tests. The level of target gene expression in developing wood of selected lines was approx. 50% of WT level for GT43B (Ratke et al., 2018), 45%-57% of WT level for GATL1.1 and 13%-25% of WT level for ASPR1 (Supplemental Figure S1). The primers for the RT-PCR analysis are listed in Supplemental Table S2.
Table 1 Lines used in this study.
2.2 Field trial establishment and phenotyping
The lines were cultivated in pots for a month at the Umeå Plant Science Centre and then planted with a 3 m spacing in August 2014 in fields located in Laholm community, Sweden (56.42 N, 13.07 E), as described previously (Derba-Maceluch et al., 2020). A permit for their planting was granted by the Swedish Board of Agriculture (DNR.4.6.18-761/14). Two trees per transgenic line and four WT trees were randomly assigned to each of 14 blocks, as shown in Supplemental Figure S2. The trial also included other transgenic lines, some of which were previously described (Derba-Maceluch et al., 2020; Pramod et al., 2021). The field was harrowed or mowed twice a year to control weeds.
Plant height was measured with a meter stick, and stem diameter was measured 3 cm from the ground with a caliper four times per year. General damage from biotic and abiotic stress was assessed using the method of Nilsson and Örlander (1999) using a 0-5 scale (no damage - dead tree) while conducting measurements. In July 2017, additional leaf biotic damage assessments were performed as described by Derba-Maceluch et al. (2020); the degree of chewing damage by arthropods (chewing) was quantified as the percentage of chewed leaves in the canopy. Other types of damage were scored in terms of presence (1) and absence (0), including damage caused by aphids, miners, gall-producing organisms, rust (Melampsora spp.), venturia (Venturia spp.), chlorosis, necrosis, and hypersensitive responses (HR). Chlorophyll content was determined with a CCM-200 plus instrument (Opti-Science, Huston, United States) on six fully developed leaves per tree for 50% of the tallest trees in each line, as previously described (Derba-Maceluch et al., 2020). The same leaves were frozen on dry ice, freeze-dried, and used for analysis of condensed tannins and phenylpropanoids (salicortin, tremulacin, salicin, tremuloidin, salicyloylsalicin, HCH-salicortin, 2′-(E)-, and 2′-(Z)-cinnamoylsalicortin, 2′-acetylsalicin, 2′-acetylsalicortin, acetyl tremulacin, HCH-2′-acetylsalicortin, and HCH-tremulacin, which are known to vary in response to biotic and abiotic stresses in Populus leaves (Keefover-Ring et al., 2014). The metabolites were analyzed as described by Derba-Maceluch et al. (2020).
In 2018 the field suffered from exceptional drought (Supplemental Figure S3) resulting in the generation of flower buds on some trees. In accordance with permit DNR.4.6.18-761/14 for field trials with transgenic trees, the field was harvested prematurely in September 2018. Stem material was collected from 50% of the tallest trees of each transgenic line and WT, including a five-cm stem segment 10 cm from the ground for SilviScan analyses and a 30-cm stem segment above it for wood chemical analyses. The segments were dried and stored at room temperature before analyses.
2.3 SilviScan analyses
SilviScan (CSIRO, Australia) measurements were conducted at RISE Research Institutes of Sweden AB using previously reported procedures (Donev et al., 2023). Briefly, wood characterization of pith to bark samples was performed on three separate measurement units to determine different properties of interest. A video microscope was used to determine the radial distribution of the numbers and sizes of fibers and vessels through image analysis. Subsequently, a high-resolution radial density profile was generated via X-ray absorption scanning. Finally, the microfibril angle at different radial positions was determined by X-ray diffraction scanning.
2.4 Stem morphology and branching
To assess differences in branching and growth morphology, trees representing the studied genotypes (N = 14) were photographed in the field before and during bud burst in May and early June of 2017. Images were analyzed using scripts written in the object-oriented programming language Python (Van Rossum and Drake, 2009) using the PlantCV library (Gehan et al., 2017). The method used is available at https://plantcv.readthedocs.io/en/stable/tutorials/vis_tutorial/. The major (a) and minor (b) axis of the ellipses fitted over the contour of each tree image are obtained, as well as the area of the tree bounding convex hull (Ach), the tree bounding box length (Lbb) and width (Wbb), and the surface area of the contour of each tree (Atree), i.e. the number of pixels corresponding to the tree. Other parameters are calculated as follows:
The number of main (primary) and secondary branches was counted manually from the images.
2.5 Wood grinding and general chemical characterization
Dry stem segments were cut into pieces roughly 5 cm long and ground in an SM 300 Cutting Mill with a 2 mm sieve (Retsch, Haan, Germany). The rough powder was then sieved using an AS 200 vibratory sieve shaker (Retsch) and divided into the following particle size fractions:< 50, 50–100, 100–500, and > 500 μm. Wood powder of each size fraction from sets of three trees was then pooled. Four such pooled samples (biological replicates) were used for each transgenic line; eight were used for the WT.
Alcohol-insoluble residue (AIR) was obtained from 10 mg of each pooled biological replicate of the 50–100 μm particle size fraction and treated with α-amylase and α-amyloglucosidase (Roche, United States) as described by Gandla et al. (2015). Approx. 50 µg portions of destarched AIR were analyzed by pyrolysis-gas chromatography/mass spectrometry (Py-GC/MS), 500 µg portions were analyzed for matrix sugar composition using an acid methanolysis-trimethylsilyl (TMS) method with two technical replicates, and approx. 3 mg were used for cellulose analysis by the Updegraff method with two technical replicates as described by Pramod et al. (2021).
All four biological replicates of the 50-100 µm sized particle fractions were pooled to obtain one pool representing 12 trees per line for transgenic trees and two pools of 12 trees each for the WT. Each pool was then analyzed in technical duplicates to determine the sugar composition by a two-step sulfuric acid hydrolysis method (Saeman et al., 1954). Aliquots (1 mg) of wood powder were incubated in 125 μL of 72% (w/v) H2SO4 at room temperature for 3 h, then diluted with 1375 μL of deionized water and incubated at 100°C for 3 h. The resulting hydrolysates were diluted with 0.9 mL of MilliQ water and filtered through a 0.2 mm syringe filter (Chromacol 17-SF-02-N) into a high-performance anion-exchange chromatography - pulsed amperometric detection (HPAEC-PAD) vial for sugar analysis.
2.6 Isolation and characterization of hemicelluloses
Hemicelluloses were purified by alkaline extraction (Timell, 1961; Escalante et al., 2012) by incubating 1 g of aspen wood powder of 12 trees, as described above, with 10 mL of a 24% (w/v) aqueous solution of KOH for 24 h at room temperature. The extract was then filtered through a 60 µm filter and neutralized by adding 0.4 volume of glacial acetic acid. Hemicellulose was precipitated with 96% (v/v) ethanol at 4°C overnight, and the precipitate was centrifuged, washed in 80% ethanol, dissolved in distilled water, and freeze-dried to obtain the hemicellulose fraction.
The sugar composition of the alkaline extracts was determined after acidic methanolysis (Bertaud et al., 2002) using 1 mg of dry extract and 1 mL of 2 M HCl in dry methanol, incubating the mixture at 100°C for 5 h. Samples were then neutralized with 200 µL of pyridine, dried under a stream of air, hydrolyzed with 2 M tri-fluoro-acetic acid (TFA) at 120°C for 1 h, air-dried, and dissolved in 1 mL milliQ water. The hydrolysates were analyzed by high-performance anion-exchange chromatography with pulsed amperometric detection (HPAEC-PAD) using a Dionex ICS-6000 instrument (Thermo Fisher Scientific, Stockholm, Sweden) equipped with a Dionex CarboPac PA1 column (4 × 250 mm) at 30°C, applying previously reported eluent gradients (McKee et al., 2016). Monosaccharide composition (monomeric form) was quantified by standard calibration of ten monosaccharides and sugar acids (Ara, Rha, Fuc, Xyl, Man, Gal, Glc, GalA, 4-O-MeGlcA and GlcA) with concentrations of 0.005 - 0.1 g/L.
The molar mass of the alkaline extracts was determined by size exclusion chromatography coupled to refractive index and UV-detectors (SECurity 1260, Polymer Standard Services, Mainz, Germany). The freeze-dried extracts were dissolved in dimethyl sulfoxide (DMSO, anhydrous, Sigma-Aldrich) to a concentration of 2 mg/mL with 0.5% w/w LiBr (Anhydrous free-flowing Redi-Dri, Sigma-Aldrich) at 60 °C overnight and filtered through 0.45 μm PTFE syringe filters (VWR). Separation was performed using GRAM Analytical columns of 100 and 10 000 Å (Polymer Standard Services, Mainz, Germany) at a flow rate of 0.5 mL/min at 60 °C. The columns were calibrated using pullulan standards between 345 and 708 000 Da (Polymer Standard Services, Mainz, Germany).
For oligosaccharide mass profiling (OLIMP), the alkali-extracted hemicelluloses were digested using GH30 endo β-(1-4) glucuronoxylanase from Bacillus subtilis (St John et al., 2006; St John et al., 2011), kindly provided by Prof. James F. Preston, University of Florida, by incubating 1 mg of dry extract in 20 mM sodium acetate buffer (pH 5.5, 1g/L) with the enzyme (10 U mL-1) for 16 h at 37 °C. After incubation, the enzyme was inactivated at 95°C and the mixture was filtered. Oligosaccharides were analyzed by liquid chromatography system (ACQUITY UPLC, Waters, USA) coupled with electron spray tandem mass spectrometer (LC-ESI-MS/MS, Synapt HDMS, Waters, USA) as described by Martínez-Abad et al. (2020). The hydrolysates were desalted with HyperSep Hypercarb cartridges (Thermo Fisher), dissolved in 50% (v/v) acetonitrile and 0.1% (v/v) formic acid, oligosaccharides were purified through a ZORBAX Eclipse Plus C18 column (1.8 µm x 2.1 mm x 50 mm, Agilent Technologies, Santa Clara, CA), and analyzed using positive ion mode in the ESI-MS. The capillary and cone voltages were set to 3 kV and 70 kV, respectively.
2.7 Analytical saccharification
Analytical enzymatic saccharification experiments were performed as described previously (Gandla et al., 2021) using 50 mg of dry wood powder (particle size 100-500 µm) from each of four biological replicates per transgenic line and ten biological replicates for WT, with two technical replicates in each case. A biological replicate consisted of pooled stem biomass from three trees. Enzymatic saccharification experiments were performed without pretreatment and with acid pretreatment. The pretreatment and enzymatic hydrolysis conditions were as described previously (Gandla et al., 2021). Briefly, pretreatment was performed in a single-mode microwave system (Initiator Exp, Biotage, Uppsala, Sweden) with sulfuric acid (1% w/w relative to the total weight of the reaction mixture) at 165 ˚C for 10 min, whereas enzymatic hydrolysis was performed in sodium citrate buffer, 50 mM, pH 5.2, using 4 mg (corresponding to approx. 3.5 μL) liquid enzyme preparation (Cellic CTec-2 obtained from Sigma-Aldrich, St. Louis, MO, U.S.A.) per sample. Cellic CTec2 has a reported protein concentration of 182 mg/mL, a cellulase activity of 77 FPU/mL, and a xylanase activity of 160 IU/mL (Qin et al., 2018). Incubation was performed at 45°C and 170 rpm (Ecotron incubator shaker, Infors, Bottmingen, Swizerland) for 72 h. Samples from reaction mixtures were centrifuged at 14 000 rpm for 10 min to separate solid and liquid portions. The glucose production rate (GPR) of the liquid portions after 2 h was determined with a glucometer (Accu-Chek® Aviva; Roche Diagnostics Scandinavia AB, Bromma, Sweden) and monosaccharide sugar yields (Ara, Gal, Glc, Xyl and Man) were determined after 72 h using a Dionex ICS-5000 HPAEC system (Thermo Fisher Scientific) with a set of standard monosaccharide sugar solutions for calibration (Wang et al., 2018).
3 Results
3.1 Growth of transgenic lines in the field
3.1.1 Survival, plant damage, and general morphology
Young trees belonging to the transgenic lines and WT were planted in the field during the summer of 2014. The mortality up to the summer of 2018 never exceeded one out of 28 trees per line (transgenic lines) or 56 trees (WT) and the survival of the modified trees therefore did not deviate from the survival of WTs (P< 0.05; Fisher’s exact test). The summer of 2018 was exceptionally dry in Southern Sweden (Supplementary Figure S3), and the entire field dried out with no surviving trees. Therefore, growth and plant damage data were only considered for the first four growing seasons up to November 2017.
During the four years of growth, many trees (30%-40%) were damaged by hares, some of them multiple times. This damage tended to occur at specific locations in the field but no significant differences were observed between the lines (Figure 1A, Supplemental Table S3). Apical shoot damage (with any cause) was observed in 20% to 40% of trees and the frequency did not differ among genotypes. Overall, 30% to 40% of the trees suffered heavy damage (corresponding to a score of 3 on a general damage scale ranging from 0 to 5) and the occurrence of damage was unrelated to genotype. This random damage affected plant growth, so to analyze effects of genotypes on growth we excluded heavily injured plants by selecting the best-growing 50% of the trees in each line.
Figure 1 Effect of genotype on plant damage and growth in the field. (A) Occurrence of injury evaluated using a general assessment scale. (B) Stem height and diameter. (C) Stem morphology parameters: solidity, elongation, ellipse eccentricity (as explained in the Material and Methods section), and number of primary and secondary branches per tree based on analyses of contour tree images. (D) Representative digitized contour images of trees. Size bar (vertical line) = 30 cm. The analyses in A, B, and C are based on 28, 14, and 7 trees per transgenic line, respectively, or 56, 28, and 14 trees for the wild-type (WT). Data in B-C are means (± SE). Asterisks denote significance assessed by Dunnett’s test for comparisons between transgenic lines and WT. (*- P<5%, ** - P<1%, *** - P<0.1%). P values indicate the significance of the difference between all lines of a construct and the WT based on contrast analysis.
Height and diameter growth were slightly reduced (by 10-13%) relative to the WT in the ASPR1 lines, especially in line 2A (Figure 1B). The lines of other transgenic constructs did not differ significantly from the WT with respect to either of these variables. The transgenic lines did not differ significantly from the WT with respect to any parameter relating to shoot morphology or tree architecture (Figures 1C, D).
Most of the transgenic lines thus exhibited growth similar to the WT and had normal morphology; only the ASPR1 construct (particularly the ASPR1_2A line) showed growth retardation.
3.1.2 Leaf damage, chlorophyll, condensed tannins, and salicinoid glycoside contents
The leaves of field-grown trees were analyzed during the summer of 2017. Biotic damage levels were relatively low in that summer: of the damage types evaluated based on presence, only rust occurred frequently (Figure 2A). Leaf damage caused by chewing arthropods was also common, and the percentage of canopy that was affected by arthropods was significantly higher in the ASPR1_2A line than in the WT and other lines (Figure 2B).
Figure 2 Leaf characteristics and damage. (A) Occurrence of injury due to different biotic factors. (B) Chewing damage showing % of canopy affected by arthropods; (C) Chlorophyll index; (D) Leaf content of different salicinoids. The data in B-D are means (± SE); n=28 transgenic and 56 wild-type (WT) trees (A, B), 13 transgenic and 25 WT trees (C) or 4 transgenic or WT trees (D). Asterisks denote significance assessed by Dunnett’s test for comparisons between transgenic lines and WT. (* P< 5%, ** P< 1%, *** P< 0.1%). P values indicate the significance of the difference between all lines of a construct and the WT based on contrast analysis.
With just one exception, there were no significant differences between genotypes with respect to leaf chlorophyll content: the ASPR1_2A line had a higher chlorophyll index than the WT (Figure 2C). Several phenolic compounds were identified in the leaves; the ASPR1 and GT43BC lines exhibited reduced levels of tremuloidin relative to the WT, and the ASPR1 line also had elevated levels of tremulacin (Figure 2D). No consistent deviations from WT levels were observed for other phenolic compounds (Supplementary Table S4).
3.2 Wood anatomy and SilviScan traits
Wood of transgenic and WT trees was analyzed using a SilviScan instrument. The annual ring width initially decreased in the ASPR1 and GT43BC lines, but by the year 2017 this behavior was only observed in the ASPR1_2A line (Figure 3A). Average wood traits were calculated for the 2015, 2016, and 2017 rings; the first ring was excluded because it was not always present in the dissected-out samples. Average annual ring area was reduced in ASPR1 lines (Figure 3B) and cell wall thickness was slightly reduced in the ASPR1 and GT43BC lines. Consequently, the wood density in these lines was slightly lower (by 5% and 6%, respectively) than in the wild type, and the GT43BC lines also exhibited reduced fiber coarseness (by 5%) (Figures 3C, E, F). The ASPR1 lines exhibited a slight increase in fiber and vessel size (Figures 3D, I), which may have contributed to their low wood density. The ASPR1 lines also exhibited a slight reduction in modulus of elasticity (MOE; by 9%) and a slight increase in cellulose microfibril angle (MFA; by 7%). Overall, these changes were very modest; the SilviScan wood traits were only slightly affected in the ASPR1 and GT43BC lines and not at all in the GATL1.1 lines.
Figure 3 Effect of genotype on wood anatomy and wood properties analyzed by SilviScan. (A) Width of the annual rings; (B) Mean ring area for years 2015-2017; (C) Mean fiber cell wall thickness. (D) Mean radial fiber diameter; (E) Mean fiber coarseness; The data are based on the best-performing 50% of trees for each line and represent means (± SE) of n=12 or 18 trees for transgenic lines and the wild-type (WT). Data for (C–H) are means for 2015-2017 growth rings (ring area weighted). Data in (A–F) are based on 25 µm resolution optical scanning. Data in (G, H) are based on 5 mm resolution X-ray diffraction scanning. Data in (I) are based on 2 mm resolution optical scanning. P values indicate the significance of the difference between all lines of a construct and the WT based on contrast analysis.
3.3 Wood chemistry
Pyrolysis-GC/MS analysis of stem biomass revealed that the biomass composition of the transgenic lines did not differ significantly from that of the WT with only one exception: the S-lignin content and S/G ratio of the ASPR1 lines were slightly reduced and their phenolic content was increased (Figure 4A). None of the transgenic lines differed significantly from the WT with respect to Updegraff cellulose content (Figure 4B). Matrix sugar content recovered by the acid methanolysis-TMS amounted to roughly 40% of the total biomass in all analyzed samples. Compared to the WT, ASPR1 lines had reduced levels of Xyl and increased levels of Fuc, Gal and GlcA (by -6%, +13%, +12% and +2%, respectively), while GT43BC lines had increased levels of Man, mGlcA and Glc (by 9%, 10% and 15%, respectively) (Figure 4C).
Figure 4 Effect of genotype on stem biomass chemical composition. (A) Relative peak integrals for compounds detected by pyrolysis-gas chromatography/mass spectrometry (Py-GC/MS). C-carbohydrates; G – guaiacyl units; S-syringyl units; H- p-hydroxyphenol units; P – phenolics: L – total lignin (G+S+H+P); (B) Updegraff cellulose content; (C) Acid methanolysis – trimethylsilyl (TMS) matrix sugar content of biomass; (D) Biomass sugar content based on two-step hydrolysis. The data are means (± SE) of n = 4 or 8 biological replicates for transgenic lines and wild-type (WT) plants, respectively (A–C) or 2 technical replicates of 12 pooled trees (D). P values indicate the significance of the difference between all lines of a construct and the WT based on contrast analysis.
When the biomass sugar composition was analyzed using two-step hydrolysis with sulfuric acid, approx. 50% of the biomass weight was recovered, with Glc and Xyl being main sugars (Figure 4D). All transgenic lines exhibited reduced levels of Xyl (by 13% to 18%) relative to the WT. In GT43BC construct lines, this effect was partially compensated by an increase in the content of Man, but the content of Glc was unaffected in agreement with the unaffected content of crystalline cellulose. All transgenic lines also exhibited strongly reduced levels of Fuc (80% to 88%), which was a minor component.
Hemicelluloses were analyzed by extracting biomass samples with a 24% KOH solution. After precipitation, this led to the recovery of 60% of the biomass weight for WT samples, but only around 50% for transgenic lines (Figure 5A) in the form of anhydrous sugars. This difference occurred because the Xyl content of the transgenic lines was 25-34% lower than in the WT. The loss of Xyl was not accompanied by any proportional loss of mGlcA; the molar ratio of Xyl to mGlcA was reduced by over 30% relative to the WT in all transgenic lines, indicating increased xylan glucuronosylation. Other changes observed in the hemicellulose sugars of the transgenic lines included strongly increased levels of GlcA (between 2 and 3.5 fold increases) in all transgenic lines, reduced levels of Glc and increased levels of Fuc in GATL1.1 and GT43BC lines, and increased levels of Gal in ASRP1 and GATL1.1 lines.
Figure 5 Effect of genotype on alkali-extracted hemicelluloses. (A) Hemicellulose sugar composition analysis by acid methanolysis - trifluoroacetic acid (TFA) high-performance anion-exchange chromatography with pulsed amperometric detection (HPAEC-PAD). The inset shows a decrease in the Xyl to mGlcA ratio in transgenic lines. P values indicate the significance of the difference between all lines of a construct and the wild-type (WT) based on contrast analysis. (B) Size exclusion analysis of hemicelluloses. (C) OLIMP analysis of alkali-extracted hemicelluloses. X-xylose unit; mU – mGlcA unit. The data in A and C are means (± SE) of n = 2 technical replicates representing 12 pooled trees.
The molecular weight distribution of hemicellulose was only slightly affected in transgenic lines (Figure 5B). All transgenic lines had a slightly increased abundance of low molecular weight polymers between 103 and 104 Da, which formed a shoulder of the main peak, and the ASPR1 and GATL1.1 construct lines also showed a shift of the main peak towards a higher molecular weight.
The profiles of oligosaccharides released by digestion with xylanase GH30, which attacks the glycosidic bond in the backbone one Xyl unit away from the mGlcA side chain towards the non-reducing end (St John et al., 2006; St John et al., 2011; Martínez-Abad et al., 2018), provided information about changes in the xylan glucuronosylation pattern in transgenic lines. The most abundant oligosaccharides were X2mU and X5mU, indicating glucuronosylation at every second and every fifth Xyl unit (Figure 5C). X3mU, X4mU, and X6mU oligosaccharides were also relatively abundant. The transgenic lines tended to have fewer X6mU units and more X3mU units than the WT. Certain lines also showed increased occurrence of X2mU units. Overall, these changes indicate a denser glucuronosylation pattern in transgenic lines compared to the WT.
3.4 Saccharification
Biomass from stems was subjected to enzymatic saccharification without pretreatment (untreated) yielding approx. 5% of biomass recovered as sugars, or to enzymatic saccharification after acid pretreatment (pretreated) with the recovery above 50% of biomass weight (Figure 6). All transgenic lines showed increased Glc production rates and Glc yields in saccharification without pretreatment. Matrix sugars were not targeted by the enzymatic mixture used here but all of them other than Xyl were released more readily from the transgenic lines than from the WT.
Figure 6 Effect of genotype on saccharification. (A) Glc production rates. (B) Sugar yields (in hydrous form) of untreated biomass and total yields after acid and enzymatic hydrolysis. Data are means (± SE), n = 4 or 10 biological replicates for each transgenic line and wild-type (WT), respectively. P values indicate the significance of the difference between all lines of a construct and the WT based on contrast analysis. Asterisks indicate means of transgenic lines differing significantly from the WT (Dunnett’s test, * – P<5%, ** – P<1%, *** – P< 0.1%.
Biomass of transgenic and WT trees gave similar yields of Xyl, Man and Glc in acid pretreatment liquid (Supplementary Figure S4). However, the ASPR1 and GATL1.1 lines gave increased yields of Ara and Gal relative to the WT. Total yields of Glc in saccharification with acid pretreatment were increased from biomass of GT43BC construct lines (by 9% on average) even though Glc production rates did not differ significantly from WT for any transgenic line. The total yields of sugars other than Ara and Gal (which were released during acid hydrolysis) were unaffected by acid pretreatment.
4 Discussion
4.1 All three constructs reduced xylan levels and altered its structure in field-grown transgenic lines
We evaluated the effects of downregulating three different classes of enzymes in field-grown hybrid aspen and found that they all affected xylan structure. GT43BC construct lines had reduced expression of two clades of glycosyl transferases from the GT43 family (Ratke et al., 2018). Suppression of these genes by 50% was previously shown to weaken xylan backbone signals relative to RES signals (indicating a chain length reduction of 5-10%) without affecting the acid methanolysis - TMS xylosyl content of cell walls under greenhouse conditions (Ratke et al., 2018). Stronger suppression (80%) of GT43B strongly reduced the xylosyl content determined by alditol acetates method (Lee et al., 2011). Under field conditions, GT43BC lines exhibited no reduction in acid methanolysis - TMS xylosyl content (Figure 4C) but did exhibit reduced Xyl unit content in HPAEC-PAD analyses of biomass subjected to two-step sulfuric acid hydrolysis and in methanolysed alkali-extracted hemicelluloses (Figure 4D, Figure 5A). Because the three sugar content analysis methods used in this work involve different depolymerization and derivatization conditions and used either destarched AIR or milled wood as their substrate, variable results would be expected. The two-step acid hydrolysis should be considered as providing a full spectrum of all sugars present in cell wall polysaccharides and it probably recovered most of the Xyl from transgenic and WT biomass. It has revealed a 13% reduction in Xyl content in transgenic lines bearing the GT43BC construct. A greater reduction of 25% in Xyl content was observed in alkaline extracts of these transgenic lines, suggesting that they have a larger fraction of alkali-insoluble xylan than the WT. Conversely, since similar amounts of Xyl were hydrolyzed by mild acid treatment in both transgenic and WT samples (Figure 4D, Supplemental Figure S4), it appears that the WT samples had relatively more acid-labile xylan. Thus, the three methods used for Xyl determination provided information about genotypic differences in xylan extractability/accessibility as well as its content. The ASPR1 and GATL1.1 transgenic lines showed similar trends in Xyl levels in all analyses performed here as the GT43BC lines, indicating that all three constructs reduced xylan levels, increased xylan resistance to alkaline extraction, and reduced xylan resistance to mild acid hydrolysis.
For all three groups of transgenic lines, the Xyl:mGlcA ratio in the hemicellulose fractions was clearly lower than in the WT and the pattern of distributions of xylo-oligosaccharides (XOS) released by GH30 indicated a reduced frequency of widely-spaced glucurosylation and an increased abundance of more tightly spaced glucuronosylation (Figures 5A, C). Thus, the xylan of all analyzed transgenic lines had increased glucuronosylation level. The xylan fraction with evenly spaced mGlcA is the dominant xylan domain and is capable of binding the hydrophilic surface of cellulose microfibrils, while the fraction with unevenly spaced mGlcA is a minor domain that cannot bind this surface (Bromley et al., 2013; Grantham et al., 2017). These two xylan domains are generated in the Golgi by the GUX1 and GUX2 clades of the GUX protein family, respectively (Bromley et al., 2013; Lyczakowski et al., 2021). None of the transgenes used in this study affected specifically any of these domains, rather they caused an overall increase in glucuronosylation (Figure 5C). This could have been driven by increased pools of UDP-Xyl in the Golgi caused by reduced rate of xylan backbone biosynthesis, creating a product-inhibition feedback for the UDP-GlcA to UDP-Xyl conversion and thus increasing the available substrate UDP-GlcA pool for GUX1 and GUX2 enzymes.
Inhibition of xylan backbone biosynthesis could also affect the backbone chain length. Xylan synthase complex mutants reportedly reduced the degree of polymerization (DP) of xylan (Peña et al., 2007; Brown et al., 2009; Lee et al., 2010; Wu et al., 2010), and a previous quantification of RES and backbone Xyl signals revealed a small reduction of backbone chain length in transgenic GT43BC hybrid aspen (Ratke et al., 2018). However, SEC analysis of alkaline-extracted hemicellulose from the same lines grown under field conditions revealed no substantial change in the xylan mass distribution (Figure 5B). This probably reflects limitations of the SEC method rather than an effect of growth conditions because the increased xylan glucuronosylation in the transgenic lines could mask small reductions in the xylan backbone DP. On the other hand, RES mutants were reported to have a broader distribution of xylan molecular weights than xylan synthase impaired plants, with some xylan having increased DP (Peña et al., 2007; Brown et al., 2009). In accordance with these reports, we observed a shift in the main hemicellulose peak to higher molecular weights and a slight enhancement of a low molecular weight shoulder in lines with suppressed GATL1.1, which probably functions in RES biosynthesis (Kong et al., 2009). Our analysis of hemicellulose sugar composition in these lines (Figure 5A) supports the involvement of Populus GATL1.1 in xylan biosynthesis. Moreover, the altered hemicellulose molecular mass profiles of these lines (Figure 5B) are consistent with the changes observed in RES mutants, suggesting that GATL1.1 plays a role in xylan RES biosynthesis.
4.2 Function of ASPR1
ASPR1 belongs to a large family of atypical aspartic proteases and nucellins. Its clade includes eight genes in P. trichocarpa and ten in Arabidopsis (Supplemental Figure S5). P. tremula has only four gene models for this family in the v 2.2 assembly, and the model for the current RNAi construct is missing. It has been suggested that the AtASPR1 cleavage site is located downstream of a leucine residue, but its specificity is unknown (Soares et al., 2019). The two other genes of this clade, AtECS1 and AtECS2, act during fertilization to prevent polytubey (Yu et al., 2021). These peptidases are secreted by fertilized ovule and hydrolyze the Cys-rich pollen tube attractant peptides LURE1.1-LURE1.5. AtASPR1 is expressed strongly in the root tips, lateral root primordia, pollen grains, and developing vascular tissue (Soares et al., 2019). Its overexpression in Arabidopsis inhibited lateral root formation and affected proteins related to biotic and abiotic stresses but its function in vascular development has not been studied. PtASPR1 is strongly induced in developing xylem during secondary wall formation (Sundell et al., 2017) suggesting involvement in secondary wall biosynthesis. The reduced Xyl content in lines with suppressed ASPR1 expression compared to WT was detectable in methanolized biomass (Figure 4A), fully hydrolyzed biomass (Figure 4B) and in alkali-extractable hemicelluloses (Figure 5A) and the levels of reduction in these lines were comparable to those seen in lines with suppressed expression of known xylan biosynthesis genes, implicating PtASPR1 in xylan biosynthesis. Moreover, the XOS profiles, the reduced Xyl to mGlcA ratio, and the molecular weight distribution of the hemicellulose fraction from the ASPR1 lines closely resembled those of GATL1.1 construct lines (Figures 5B, C). These observations suggest that ASPR1 may regulate xylan RES biosynthesis.
4.3 Evaluation of trait stability under greenhouse and field conditions
There were both drastic (Taniguchi et al., 2012; Dominguez et al., 2021) and modest (Derba-Maceluch et al., 2020; Pramod et al., 2021) differences in the performance of the transgenic trees when comparing greenhouse and field conditions. Because the GT43BC lines tested in the field in this work were previously studied under greenhouse conditions (Ratke et al., 2018), it was possible to evaluate the stability of several of their traits. Some traits showed high stability under both growth conditions – for example, the transgenic lines exhibited reduced secondary wall thickness and wood density, increased acid methanolysis - TMS Man contents, and unchanged acid methanolysis - TMS Xyl contents as well as improved biomass saccharification properties in enzymatic saccharification without pretreatment in the field (Figures 3C, F, 4C, 6A, B) and the greenhouse (Ratke et al., 2018). However, other traits were not reproduced under field conditions. For example, the S-lignin content and S/G ratio of field-grown transgenic trees did not differ from those in the WT but were reduced under greenhouse conditions. The highly improved growth phenotype observed in the greenhouse experiments (Ratke et al., 2018) was also not reproduced in the field (Figures 1B, 2A). The improvements in Glc yields during saccharification without pretreatment were also lower than expected based on the greenhouse experiments (16% and 8% versus 27% and 40% for line 11 and 18, respectively) (Figure 6B). However, the field- grown lines exhibited a 9% improvement in saccharification yields after acid pretreatment that was not observed in the greenhouse. Thus, some traits of transgenic trees were stable regardless of the growth conditions while others changed in the field.
4.4 Evaluation of transgenic lines as potential biorefinery feedstocks from short-rotation plantations
In the field, the GATL1.1 and GT43BC construct lines did not differ from the WT with respect to any productivity parameters relating to growth, morphology, biotic damage, or the chlorophyll index. However, ASPR1 lines exhibited mildly reduced growth (an 11% reduction in height and diameter) as well as a higher chlorophyll index and more extensive chewing damage (Figures 1, 2). These lines also showed the most pronounced reduction in Xyl content (Figures 3C, D, 5A). Levels of foliar tannins and salicinoid glucosides were generally unaltered in the transgenic lines, but the GT43BC and ASPR1 construct lines exhibited reduced levels of tremuloidin and the ASPR1 lines exhibited elevated levels of tremulacin (Figure 2D, Supplementary Table S3). These differences in salicinoid phenolic glycosides could potentially have affected the plants’ relationships with antagonists (Cole et al., 2021), but we found no evidence of any direct relationship. The wood anatomical traits of the transgenic lines were generally unaltered except for small (5%-7%) reductions in cell wall thickness and wood density in GT43BC and ASPR1 lines as well as a reduced MOE in ASPR1 construct lines, which was probably due to their increased MFA (Figures 3C, E-H). A substantial decrease in secondary wall thickness was also reported for xylan biosynthetic mutants and transgenic lines with reduced expression of xylan biosynthetic genes in which xylan content was decreased (Zhou et al., 2006; Brown et al., 2007; Lee et al., 2007b; Brown et al., 2009; Lee et al., 2011; Wu et al., 2009; Wu et al., 2010; Li et al., 2011). This decrease was previously attributed directly to their reduced xylan content. However, an analysis of transcriptomic changes in developing wood of GT43BC construct lines revealed that the suppression of the GT43 clade B and C genes caused a downregulation of the entire secondary wall biosynthetic program (Ratke et al., 2018). Moreover, the relatively slight reduction in Xyl content observed in transgenic lines, considering that xylan constitutes only one fourth of cell wall biomass, is unlikely to induce noticeable change in cell wall thickness. The reduced cell wall thickness seen in ASPR1 construct lines in this study, similar to cell wall thickness reductions in GT43BC lines, supports the hypothesis that xylan deficiency in secondary walls may affect secondary wall biosynthesis more generally.
Considering the potential of the studied lines as biorefinery feedstocks, we found that all constructs improved Glc yields in saccharification without pretreatment (Figures 6A, B). The overview of changes in most relevant productivity and saccharification traits of transgenic lines is shown in Figure 7. The best lines of each transgene, ASPR1_3A, GATL1.1_1A, and GT43BC_11, provided Glc yield increases of 13%, 19% and 16%, respectively. However, only GT43BC construct lines provided improved Glc yields of saccharification with acid pretreatment, with the best line giving a 15% increase. As neither cellulose content not matrix Glc content (except for GT43BC_11) were increased in these lines, this indicated that the genetic change that resulted in decreased xylan content in these lines lead to an altered cell wall architecture and higher accessibility of saccharification enzymes to substrates. In the case of GT43BC lines, the increased accessibility was also observed after acid pretreatment, which is of particular interest considering the presence of the pretreatment step in current technologies. Because these lines exhibit normal growth but some have slightly lower wood density than WT plants, these higher Glc yields should result in modestly improved total Glc gains per hectare.
Figure 7 Overview of most important traits that were improved or deteriorated in the field-grown transgenic lines compared to wild-type.
Data availability statement
The original contributions presented in the study are included in the article/Supplementary Material. Further inquiries can be directed to the corresponding author.
Author contributions
MD-M overviewed field trial setting up and phenotyping in 2017. PS carried out wood grinding and chemical analyses with help of RV and EH and supervision of FV and EM. ED carried out statistical analyses, data plotting and prepared the figures. MG and LJ were responsible for pretreatment and saccharification analyses. ZY and GS were responsible for SilviScan analyses. UJ was responsible for field management, operation and phenotyping. FA and BA were responsible for biotic stress estimation in 2017 and leaf phenotyping. MH produced and selected transgenic lines for field testing, EM coordinated the study, ensured the funding and wrote the paper with contributions from all the authors. All authors contributed to the article and approved the submitted version.
Funding
This work was supported by Bio4Energy (https://bio4energy.se) and the SSF program ValueTree RBP14-0011 to EM, and by grants from the Swedish Governmental Agency for Innovation Systems) and KAW (The Knut and Alice Wallenberg Foundation), and by TC4F project supporting UPSC facilities. FV acknowledges the Swedish Research Council (Project Grant 2020-04720) and the Wallenberg Wood Science Centre funded by KAW for financial support to PS and EH, respectively.
Acknowledgments
The authors thank Dr. J. Takahashi-Schmidt of the Biopolymer Analytical Platform of KBC at Umeå University for help with cell wall analyses and the Swedish Metabolomic Centre in Umeå for carrying out metabolite analyses, and Prof. James F. Preston, University of Florida for the gift of GH30.
Conflict of interest
Author MH was employed by company SweTree Technologies AB.
The remaining 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.
Publisher’s note
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.
Supplementary material
The Supplementary Material for this article can be found online at: https://www.frontiersin.org/articles/10.3389/fpls.2023.1218302/full#supplementary-material
Supplementary Figure 1 | Expression levels of targeted genes in developing wood tissues.
References
Anders, N., Wilson, L. F. L., Sorieul, M., Nikolovski N and Dupree, P. (2023). β-1,4-Xylan backbone synthesis in higher plants: how complex can it be? front. Plant Sci. 13. doi: 10.3389/fpls.2022.1076298
Bar-On, Y. M., Phillips, R., Milo, R. (2018). The biomass distribution on earth. Proc. Natl. Acad. Sci. U.S.A. 115, 6506–6511. doi: 10.1073/pnas.1711842115
Bertaud, F., Sundberg, A., Holmbom, B. (2002). Evaluation of acid methanolysis for analysis of wood hemicelluloses and pectins. Carbohydr. Polymers 48, 319–324. doi: 10.1016/S0144-8617(01)00249-1
Biswal, A. K., Hao, Z., Pattathil, S., Yang, X., Winkeler, K., Collins, C., et al (2015). Downregulation of GAUT12 in Populus deltoides by RNA silencing results in reduced recalcitrance, increased growth and reduced xylan and pectin in a woody biofuel feedstock. Biotechnology for biofuels, 8–14. doi: 10.1186/s13068-015-0218-y
Bromley, J. R., Busse-Wicher, M., Tryfona, T., Mortimer, J. C., Zhang, Z., Brown, D. M., et al. (2013). GUX1 and GUX2 glucuronyltransferases decorate distinct domains of glucuronoxylan with different substitution patterns. Plant J. 74, 423–434. doi: 10.1111/tpj.12135
Brown, D. M., Goubet, F., Wong, V. W., Goodacre, R., Stephens, E., Dupree, P., et al. (2007). Comparison of five xylan synthesis mutants reveals new insight into the mechanisms of xylan synthesis. Plant J. 52, 1154–1168. doi: 10.1111/j.1365-313X.2007.03307.x
Brown, D. M., Zhang, Z., Stephens, E., Dupree, P., Turner, S. R. (2009). Characterization of IRX10 and IRX10-like reveals an essential role in glucuronoxylan biosynthesis in arabidopsis. Plant J. 57 (4), 732–746. doi: 10.1111/j.1365-313X.2008.03729.x
Cole, C. T., Morrow, C. J., Barker, H. L., Rubert-Nason, K. F., Riehl, J. F. L., Köllner, T. G., et al. (2021). Growing up aspen: ontogeny and trade-offs shape growth, defence and reproduction in a foundation species. Ann. Bot. 127 (4), 505–517. doi: 10.1093/aob/mcaa070
Derba-Maceluch, M., Amini, F., Donev, E. N., Pawar, P. M.-A., Michaud, L., Johansson, U., et al. (2020). Cell wall acetylation in hybrid aspen affects field performance, foliar phenolic composition and resistance to biological stress factors in a construct-dependent fashion. Front. Plant Sci. 11. doi: 10.3389/fpls.2020.00651
Dominguez, P. G., Donev, E., Derba-Maceluch, M., Bünder, A., Hedenström, M., Tomášková, I., et al. (2021). Sucrose synthase determines carbon allocation in developing wood and alters carbon flow at the whole tree level in aspen. New Phytol. 229, 186–198. doi: 10.1111/nph.16721
Donev, E. N., Derba-Maceluch, M., Yassin, Z., Gandla, M. L., Pramod, S., Heinonen, E., et al. (2023). Field testing of transgenic aspen from large greenhouse screening identifies unexpected winners. Plant Biotechnol. J. 21 (5), 1005–1021. doi: 10.1111/pbi.14012
Donev, E., Gandla, M. L., Jönsson, L. J., Mellerowicz, E. J. (2018). Engineering non-cellulosic polysaccharides of wood for the biorefinery. Front. Plant Sci. 9. doi: 10.3389/fpls.2018.01537
Escalante, A., Gonçalves, A., Bodin, A., Stepan, A., Sandström, C., Toriz, G., et al. (2012). Flexible oxygen barrier films from spruce xylan. Carbohydr. Polym. 87, 2381–2387. doi: 10.1016/j.carbpol.2011.11.003
Gandla, M. L., Derba-Maceluch, M., Liu, X., Gerber, L., Master, E. R., Mellerowicz, E. J., et al. (2015). Expression of a fungal glucuronoyl esterase in Populus: effects on wood properties and saccharification efficiency. Phytochemistry 112, 210–220. doi: 10.1016/j.phytochem.2014.06.002
Gandla, M. L., Mähler, N., Escamez, S., Skotare, T., Obudulu, O., Möller, L., et al. (2021). Overexpression of vesicle-associated membrane protein PttVAP27-17 as a tool to improve biomass production and the overall saccharification yields in Populus trees. Biotechnol. Biofuels 14, 43. doi: 10.1186/s13068-021-01895-0
Gehan, M. A., Fahlgren, N., Abbasi, A., Berry, J. C., Callen, S. T., Chavez, L., et al. (2017). PlantCV v2: image analysis software for high-throughput plant phenotyping. PeerJ 5, e4088. doi: 10.7717/peerj.4088
Grantham, N. J., Wurman-Rodrich, J., Terrett, O. M., Lyczakowski, J. J., Stott, K., Iuga, D., et al. (2017). An even pattern of xylan substitution is critical for interaction with cellulose in plant cell walls. Nat. Plants 3, 859–865. doi: 10.1038/s41477-017-0030-8
Jensen, J. K., Kim, H., Cocuron, J. C., Orler, R., Ralph, J., Wilkerson, C. G., et al (2011). The DUF579 domain containing proteins IRX15 and IRX15-L affect xylan synthesis in Arabidopsis. Plant J. 66 (3), 387–400. doi: 10.1111/tpj.12641
Jensen, J. K., Johnson, N. R., Wilkerson, C. G. (2014). Arabidopsis thaliana IRX10 and two related proteins from psyllium and physcomitrella patens are xylan xylosyltransferases. Plant J. 80, 207–215. doi: 10.1111/tpj.12641
Jiang, N., Wiemels, R. E., Soya, A., Whitley, R., Held, M., Faik, A. (2016). Composition, assembly, and trafficking of a wheat xylan synthase complex. Plant Physiol. 170, 1999–2023. doi: 10.1104/pp.15.01777
Jönsson, L. J., Martín, C. (2016). Pretreatment of lignocellulose: formation of inhibitory by-products and strategies for minimizing their effects. Bioresour Technol. 199, 103–112. doi: 10.1016/j.biortech.2015.10.009
Karimi, M., Inzé, D., Depicker, A. (2002). GATEWAYTM vectors for agrobacterium mediated plant transformation. Trends Plant Sci. 7, 193–195. doi: 10.1016/S1360-1385(02)02251-3
Keefover-Ring, K., Ahnlund, M., Abreu, I. N., Jansson, S., Moritz, T., Albrectsen, B. R. (2014). No evidence of geographical structure of salicinoid chemotypes within Populus tremula. PloS One 9, e107189. doi: 10.1371/journal.pone.0107189
Kong, Y., Zhou, G., Avci, U., Gu, X., Jones, C., Yin, Y., et al. (2009). Two poplar glycosyltransferase genes, PdGATL1.1 and PdGATL1.2, are functional orthologs to PARVUS/AtGATL1 in arabidopsis. Mol. Plant 2, 1040–1050. doi: 10.1093/mp/ssp068
Kumar, V., Hainaut, M., Delhomme, N., Mannapperuma, C., Street, N. R., Henrissat, B., et al. (2019). Poplar carbohydrate-active enzymes: new annotation and functional analyses based on RNA expression data. Plant J. 99, 598–609. doi: 10.1111/tpj.14417
Lee, C., O'Neill, M. A., Tsumuraya, Y., Darvill, A. G., Ye, Z. H. (2007a). The irregular xylem9 mutant is deficient in xylan xylosyltransferase activity. Plant Cell Physiol. 48, 1624–1634. doi: 10.1093/pcp/pcm135
Lee, C., Zhong, R., Richardson, E. A., Himmelsbach, D. S., McPhail, B. T., Ye, Z. H. (2007b). The PARVUS gene is expressed in cells undergoing secondary wall thickening and is essential for glucuronoxylan biosynthesis. Plant Cell Physiol. 48, 1659–1672. doi: 10.1093/pcp/pcm155
Lee, C., Zhong, R., Ye, Z. H. (2012). Biochemical characterization of xylan xylosyltransferases involved in wood formation in poplar. Plant Signal Behav. 7 (3), 332–337. doi: 10.4161/psb.19269
Lee, C., Teng, Q., Huang, W., Zhong, R., Ye, Z. H. (2009a). The poplar GT8E and GT8F glycosyltransferases are functional orthologs of arabidopsis PARVUS involved in glucuronoxylan biosynthesis. Plant Cell Physiol. 50, 1982–1987. doi: 10.1093/pcp/pcp131
Lee, C., Teng, Q., Huang, W., Zhong, R., Ye, Z.-H. (2009b). Downregulation of PoGT47C expression in poplar results in a reduced glucuronoxylan content and an increased wood digestibility by cellulase. Plant Cell Physiol. 50, 1075–1089. doi: 10.1093/pcp/pcp060
Lee, C., Teng, Q., Huang, W., Zhong, R., Ye, Z. H. (2010). The arabidopsis family GT43 glycosyltransferases form two functionally nonredundant groups essential for the elongation of glucuronoxylan backbone. Plant Physiol. 153, 526–541. doi: 10.1104/pp.110.155309
Lee, C., Teng, Q., Zhong, R., Ye, Z. H. (2011). Molecular dissection of xylan biosynthesis during wood formation in poplar. Mol. Plant 4, 730–747. doi: 10.1093/mp/ssr035
Li, Q., Min, D., Wang, J. P., Peszlen, I., Horvath, L., Horvath, B., et al. (2011). Down-regulation of glycosyltransferase 8D genes in Populus trichocarpa caused reduced mechanical strength and xylan content in wood. Tree Physiol. 31, 226–236. doi: 10.1093/treephys/tpr008
Lyczakowski, J. J., Yu, L., Terrett, O. M., Fleischmann, C., Temple, H., Thorlby, G., et al (2021). Two conifer GUX clades are responsible for distinct glucuronic acid patterns on xylan. New Phytologist 231 (5), 1720–1733. doi: 10.1111/nph.17531
Martínez-Abad, A., Jimeínez-Quero, A., Wohlert, J., Vilaplana, F. (2020). Influence of the molecular motifs of mannan and xylan populations on their recalcitrance and organization in spruce softwoods. Green Chem. 22, 3596–3970. doi: 10.1039/D0GC01207F
Martínez-Abad, A., Giummarella, N., Lawoko, M., Vilaplana, F. (2018). Differences in extractability under subcritical water reveal interconnected hemicellulose and lignin recalcitrance in birch hardwoods. Green Chem. 20, 2534–2546. doi: 10.1039/c8gc00385h
McKee, L. S., Sunner, H., Anasontzis, G. E., Toriz, G., Gatenholm, P., Bulone, V., et al. (2016). GH115 α-glucuronidase from Schizophyllum commune contributes to the synergistic enzymatic deconstruction of softwood glucuronoarabinoxylan. Biotechnol. Biofuels 9, 2. doi: 10.1186/s13068-015-0417-6
Nilsson, U., Örlander, G. (1999). Vegetation management on grass-dominated clearcuts planted with Norway spruce in southern Sweden. Can. J. For. Res. 29, 1015–1026. doi: 10.1139/x99-071
Peña, M. J., Zhong, R., Zhou, G. K., Richardson, E. A., O'Neill, M. A., Darvill, A. G., et al. (2007). Arabidopsis irregular xylem8 and irregular xylem9: implications for the complexity of glucuronoxylan biosynthesis. Plant Cell 19, 549–563. doi: 10.1105/tpc.106.049320
Pramod, S., Gandla, M. L., Derba-Maceluch, M., Jönsson, L. J., Mellerowicz, E. J., Winestrand, S. (2021). Saccharification potential of transgenic greenhouse- and field-grown aspen engineered for reduced xylan acetylation. Front. Plant Sci. 12. doi: 10.3389/fpls.2021.704960
Qin, L., Zhao, X., Li, W.-C., Zhu, J.-Q., Liu, L., Li, B. Z., et al. (2018). Process analysis and optimization of simultaneous saccharification and co−fermentation of ethylenediamine−pretreated corn stover for ethanol production. Biotechnol. Biofuels 11, 118. doi: 10.1186/s13068-018-1118-8
Ratke, C., Pawar, P. M., Balasubramanian, V. K., Naumann, M., Duncranz, M. L., Derba-Maceluch, M., et al. (2015). Populus GT43 family members group into distinct sets required for primary and secondary wall xylan biosynthesis and include useful promoters for wood modification. Plant Biotechnol. J. 13, 26–37. doi: 10.1111/pbi.12232
Ratke, C., Terebieniec, B. K., Winestrand, S., Derba-Maceluch, M., Grahn, T., Schiffthaler, B., et al. (2018). Downregulating aspen xylan biosynthetic GT43 genes in developing wood stimulates growth via reprograming of transcriptome. New Phytol. 219, 230–245. doi: 10.1111/nph.15160
Saeman, J. F., Moore, W. E., Mitchell, R. L., Millett, M. A. (1954). Techniques for the determination of pulp constituents by quantitative paper chromatography. Tappi J. 37, 336–343.
Scheller, H. V., Ulvskov, P. (2010). Hemicelluloses. Annu. Rev. Plant Biol. 61, 263–289. doi: 10.1146/annurev-arplant-042809-112315
Smith, P. J., Wang, H. T., York, W. S., Peña, M. J., Urbanowicz, B. R. (2017). Designer biomass for next-generation biorefineries: leveraging recent insights into xylan structure and biosynthesis. Biotechnology for biofuels 10, 286. doi: 10.1186/s13068-017-0973-z
Soares, A., Niedermaier, S., Faro, R., Loos, A., Manadas, B., Faro, C., et al. (2019). An atypical aspartic protease modulates lateral root development in arabidopsis thaliana. J. Exp. Bot. 70, 2157–2171. doi: 10.1093/jxb/erz059
St John, F. J., Hurlbert, J. C., Rice, J. D., Preston, J. F., Pozharski, E. (2011). Ligand bound structures of a glycosyl hydrolase family 30 glucuronoxylan xylanohydrolase. J. Mol. Biol. 407, 92–109. doi: 10.1016/j.jmb.2011.01.010
St John, F. J., Rice, J. D., Preston, J. F. (2006). Characterization of XynC from bacillus subtilis subsp. subtilis strain 168 and analysis of its role in depolymerization of glucuronoxylan. J. Bacteriol. 188 (24), 8617–8626. doi: 10.1128/JB.01283-06
Sundell, D., Street, N. R., Kumar, M., Mellerowicz, E. J., Kucukoglu, M., Johnsson, C., et al. (2017). AspWood: high-spatial-resolution transcriptome profiles reveal uncharacterized modularity of wood formation in populus tremula. Plant Cell 29, 1585–1604. doi: 10.1105/tpc.17.00153
Taniguchi, T., Konagaya, K., Kurita, M., Takata, N., Ishii, K., Kondo, T., et al. (2012). Growth and root sucker ability of field-grown transgenic poplars overexpressing xyloglucanase. J. Wood Sci. 58, 550–556. doi: 10.1007/s10086-012-1281-7
Timell, T. E. (1961). Isolation of galactoglucomannans from the wood of gymnosperms. Tappi J. 44 (2), 88–96.
Wang, Z., Winestrand, S., Gillgren, T., Jönsson, L. J. (2018). Chemical and structural factors influencing enzymatic saccharification of wood from aspen, birch and spruce. Biomass Bioenergy 109, 125–134. doi: 10.1016/j.biombioe.2017.12.020
Wierzbicki, M. P., Maloney, V., Mizrachi E and Myburg, A. A. (2019). Xylan in the middle: understanding xylan biosynthesis and its metabolic dependencies toward improving wood fiber for industrial processing. Front. Plant Sci. 10. doi: 10.3389/fpls.2019.00176
Wu, A. M., Rihouey, C., Seveno, M., Hörnblad, E., Singh, S. K., Matsunaga, T., et al. (2009). The Arabidopsis IRX10 and IRX10-LIKE glycosyltransferases are critical for glucuronoxylan biosynthesis during secondary cell wall formation. Plant J. 57 (4), 718–731. doi: 10.1111/j.1365-313X.2008.03724.x
Wu, A. M., Hörnblad, E., Voxeur, A., Gerber, L., Rihouey, C., Lerouge, P., et al. (2010). Analysis of the arabidopsis IRX9/IRX9-l and IRX14/IRX14-l pairs of glycosyltransferase genes reveals critical contributions to biosynthesis of the hemicellulose glucuronoxylan. Plant Physiol. 153, 542–554. doi: 10.1104/pp.110.154971
Yu, X., Zhang, X., Zhao, P., Peng, X., Chen, H., Bleckmann, A., et al. (2021). Fertilized egg cells secrete endopeptidases to avoid polytubey. Nature 592, 433–437. doi: 10.1038/s41586-021-03387-5
Zeng, W., Lampugnani, E. R., Picard, K. L., Song, L., Wu, A. M., Farion, I. M., et al. (2016). Asparagus IRX9, IRX10, and IRX14A are components of an active xylan backbone synthase complex that forms in the golgi apparatus. Plant Physiol. 171, 93–109. doi: 10.1104/pp.15.01919
Zhou, G. K., Zhong, R., Himmelsbach, D. S., McPhail, B. T., Ye, Z. H. (2007). Molecular characterization of PoGT8D and PoGT43B, two secondary wall-associated glycosyltransferases in poplar. Plant Cell Physiol. 48, 689–699. doi: 10.1093/pcp/pcm037
Keywords: field trial, GMO, Populus tremula x tremuloides, saccharification, salicinoid phenolic glucosides, SilviScan, transgenic trees, xylan
Citation: Derba-Maceluch M, Sivan P, Donev EN, Gandla ML, Yassin Z, Vaasan R, Heinonen E, Andersson S, Amini F, Scheepers G, Johansson U, Vilaplana FJ, Albrectsen BR, Hertzberg M, Jönsson LJ and Mellerowicz EJ (2023) Impact of xylan on field productivity and wood saccharification properties in aspen. Front. Plant Sci. 14:1218302. doi: 10.3389/fpls.2023.1218302
Received: 06 May 2023; Accepted: 27 June 2023;
Published: 17 July 2023.
Edited by:
Gabriel Paes, l’alimentation et l’environnement (INRAE), FranceReviewed by:
Maija Tenkanen, University of Helsinki, FinlandWei Zeng, Zhejiang Agriculture and Forestry University, China
Copyright © 2023 Derba-Maceluch, Sivan, Donev, Gandla, Yassin, Vaasan, Heinonen, Andersson, Amini, Scheepers, Johansson, Vilaplana, Albrectsen, Hertzberg, Jönsson and Mellerowicz. 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) and the copyright owner(s) 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: Ewa J. Mellerowicz, ewa.mellerowicz@slu.se