Skip to main content
  • Research article
  • Open access
  • Published:

Partial functional conservation of IRX10 homologs in physcomitrella patens and Arabidopsis thalianaindicates an evolutionary step contributing to vascular formation in land plants

Abstract

Background

Plant cell walls are complex multicomponent structures that have evolved to fulfil an essential function in providing strength and protection to cells. Hemicelluloses constitute a key component of the cell wall and recently a number of the genes thought to encode the enzymes required for its synthesis have been identified in Arabidopsis. The acquisition of hemicellulose synthesis capability is hypothesised to have been an important step in the evolution of higher plants.

Results

Analysis of the Physcomitrella patens genome has revealed the presence of homologs for all of the Arabidopsis glycosyltransferases including IRX9, IRX10 and IRX14 required for the synthesis of the glucuronoxylan backbone. The Physcomitrella IRX10 homolog is expressed in a variety of moss tissues which were newly formed or undergoing expansion. There is a high degree of sequence conservation between the Physcomitrella IRX10 and Arabidopsis IRX10 and IRX10-L. Despite this sequence similarity, the Physcomitrella IRX10 gene is only able to partially rescue the Arabidopsis irx10 irx10-L double mutant indicating that there has been a neo- or sub-functionalisation during the evolution of higher plants. Analysis of the monosaccharide composition of stems from the partially rescued Arabidopsis plants does not show any significant change in xylose content compared to the irx10 irx10-L double mutant. Likewise, knockout mutants of the Physcomitrella IRX10 gene do not result in any visible phenotype and there is no significant change in monosaccharide composition of the cell walls.

Conclusions

The fact that the Physcomitrella IRX10 (PpGT47A) protein can partially complement an Arabidopsis irx10 irx10-L double mutant suggests that it shares some function with the Arabidopsis proteins, but the lack of a phenotype in knockout lines shows that the function is not required for growth or development under normal conditions in Physcomitrella. In contrast, the Arabidopsis irx10 and irx10 irx10-L mutants have strong phenotypes indicating an important function in growth and development. We conclude that the evolution of vascular plants has been associated with a significant change or adaptation in the function of the IRX10 gene family.

Background

The components and structures of plant cell walls have evolved over millions of years, resulting in a diverse range of traits and functions. From a comparison of cell walls of land plants, it is apparent that there are some common structural components, and that at least a proportion of the cell wall biosynthesis machinery is likely to be conserved among embryophytes. Studies have shown that members of the charophycean green algae, the closest relatives of land plants, possess cell walls that share many basic components with the embryophyte primary cell wall including a number of polysaccharides, structural proteins and lignin [1–3]. Although some of the components of the plant cell wall may have formed via convergent evolution, it seems likely that others were present in a common ancestor and were retained following colonisation of the land by plants. It can be hypothesised that glycosyltransferases (GTs) required for synthesis of some of the cell wall polysaccharides will be conserved between lower and higher plants.

Comparative biochemical analyses based on enzymatic digestion, linkage analyses and immunolocalisation of polysaccharide epitopes have been used to show similarities and differences between the cell wall components of angiosperms and bryophytes [1, 4–9]. Some bryophyte cell wall polymers including cellulose, glucuronoxylan and rhamnogalacturonan II have been isolated and characterized [4, 10–12], but very little is known about the evolutionary relationship between the genes encoding the enzymes required for cell wall biosynthesis in lower and higher plants. The cell wall organisation of Physcomitrella patens is similar to the angiosperm primary cell wall and almost all major non-lignin cell wall components including cellulose, hemicelluloses (except xylogalacturonan), pectins and arabinogalactan proteins (AGPs) found in angiosperms are also present in bryophytes though in different proportions. There are however some components such as mixed-linkage β-glucans which are found in some land plants but not in the bryophytes.

Cell walls of higher plants have significantly more xylan than lower plants such as the bryophytes indicating that a change in the proportion of the hemicellulose polymer present in cell walls may have been a key step in plant evolution [6, 9, 12, 13]. The hemicellulose glucuronoxylan (GX) is the second most abundant polymer in hardwood secondary cell walls, and is a major component of dicot wood [14, 15]. There is a high degree of conservation of both the GX biosynthesis machinery and the structure of GX between Arabidopsis and Populus[16–22], but it is only recently that equivalent information has been obtained from lower plants including bryophytes [12].

The structure of GX in angiosperm secondary cell walls is highly conserved consisting of a partly acetylated β-D-(1 → 4)-Xylp backbone substituted with either 4-O-methylated (Me)- or non-methylated glucuronic acid (GlcpA) side chains [23]. Analysis of GX from spruce, birch, aspen and Arabidopsis has revealed a conserved oligosaccharide at the reducing end comprised of β-D-Xylp-(1 → 3)-α-L-Rhap-(1 → 2)-α-D-GalpA-(1 → 4)-D-Xyl [14, 23–28]. In the moss Physcomitrella patens, a xylan polymer substituted at the O-2 position by α-D-GlcpA has been detected. However, in contrast to higher plants the moss xylan was not substituted by 4-O-Me GlcpA and the presence of a reducing end oligosaccharide was also not detected [12]. Twelve glycosyltransferase genes have been identified to date in Arabidopsis that are involved in GX synthesis; namely IRREGULAR XYLEM 10 (AtIRX10), AtIRX10-Like (AtIRX10-L), AtIRX9, AtIRX9-L, AtIRX14, AtIRX14-L, AtFRAGILE FIBER 8 (AtFRA8), AtFRAGILE FIBER 8 HOMOLOG (AtF8H), AtIRX8, AtPARVUS, AtGUX1 and AtGUX2[19, 29–39]. Although enzymatic activity has yet to be demonstrated for any of the putative GX synthesis enzymes, microsome experiments support the hypothesis that AtIRX9, AtIRX10 and AtIRX14 are involved in synthesis of the β-D-(1 → 4)-xylan backbone [33, 40, 41] while the AtIRX8, AtPARVUS and AtFRA8 enzymes are instead thought to function to synthesise the reducing end oligosaccharide [19, 31, 32]. Evidence for conservation of the GX biosynthetic machinery between herbaceous and woody plants has come from the finding that Populus homologs of putative Arabidopsis GX synthesis enzymes are able to complement the corresponding Arabidopsis mutants [16–18, 22, 42]. Two Populus IRX10 homologs have been shown to be functionally conserved with the Arabidopsis IRX10 homolog as they can fully restore the Arabidopsis irx10 irx10-L double mutant to a wild-type phenotype (Hörnblad & Marchant, unpublished data).

In this study, Physcomitrella has been used to investigate the origin and functional role of the GT47 or IRX10 gene family. Results obtained suggest a common ancestor for the IRX10 gene family in Populus, Arabidopsis and Physcomitrella, and supports a partial conservation of the components in the GX biosynthetic machinery. In Arabidopsis and Populus, expression of a number of IRX10 gene family members is strongly correlated with the vasculature whereas expression in Physcomitrella is found in tissues undergoing expansion rather than in water-conducting cells. Furthermore, the lack of increased xylose content in the Arabidopsis irx10 irx10-L double knockout plants complemented with PpGT47A reveal that although the proteins are likely to share a common genetic origin, they are no longer directly functionally interchangeable.

Results

The Physcomitrellagenome contains genes encoding homologs of all known enzymes involved in synthesis of the glucuronoxylan backbone

Work carried out in Arabidopsis has shown that there are multiple enzymes involved in the synthesis of the glucuronoxylan backbone (IRX9, IRX10 and IRX14), substitution of the backbone (GUX1/GUX2) and synthesis of the reducing end oligosaccharide (IRX8, FRA8 and PARVUS) [30, 31, 40]. To determine whether there is conservation of the genes required for xylan biosynthesis between higher and lower plants, each of the Arabidopsis proteins proposed to function in the synthesis of glucuronoxylan were used to BLAST search the Physcomitrella genome. A single putative IRX10 homolog is present in Physcomitrella encoded by Pp1s7_455V6 (PpGT47A) (Table 1) which shows a high degree of conservation with the Arabidopsis and Populus trichocarpa IRX10 proteins (Figure 1). The N-terminal regions of the Arabidopsis and Populus IRX10 proteins are the most divergent domains and contain predicted signal peptides in AtIRX10, AtIRX10-L, PtGT47A-1 and PtGT47A-2 whereas the N-terminal region of PpGT47A has a predicted transmembrane domain in common with two of the other Populus homologs PtGT47D-1 and PtGT47D-4 [43, 44] (Table 2). Two putative homologs were found for AtIRX9/IRX9-L (Pp1s52_108V6.1 and Pp1s1_540V6.1), whereas three putative homologs were each identified for AtIRX14/IRX14-L (Pp1s248_13V6.1, Pp1s78_128V6.1 and Pp1s19_221V6.1), AtFRA8/F8H (Pp1s13_216V6.1, Pp1s217_58V6.2 and Pp1s315_20V6.1), and AtGUX1/GUX2 (Pp1s21_381V6.1, Pp1s351_36V6.1 and Pp1s223_30V6.1) (Figure 2). Interestingly, there were no closely related sequences found for AtIRX8. Although several sequences were identified that exhibited a 60% similarity with PARVUS, all of them exhibited a higher degree of similarity with other Arabidopsis proteins and so were not considered likely to be homologs of PARVUS (Table 1). The degree of similarity between the Arabidopsis and Physcomitrella homologs was between 25% and 48% except in the case of the PpGT47A which exhibited 76% similarity with AtIRX10 and AtIRX10-L. All genes are present in two or three copies encoding closely related proteins in both species, with the exception of PpGT47A which is unique (Figure 2). In all cases, duplicated or triplicated genes within a species encode proteins that cluster together (Figure 2). This suggests that gene duplications have occurred in both species after they split from each other. However, concerted evolution of related genes cannot be ruled out as a reason for close similarity, at least not in Physcomitrella, where it has been previously observed [45]. The high degree of sequence similarity exhibited between the Arabidopsis IRX10 and the Physcomitrella GT47A proteins further suggests that they may exhibit functional conservation and thus may give clues as to the evolutionary origin of the GX biosynthesis machinery in higher plants.

Table 1 Similarity between the Arabidopsis GX synthesis proteins and their respective Arabidopsis and Physcomitrella homologs
Figure 1
figure 1

Sequence alignment of the Arabidopsis , Populus and Physcomitrella IRX10 protein family. IRX10 related protein sequences from Arabidopsis, Populus and Physcomitrella were aligned using Clustal-X. Shading indicates 100% conservation (black), 80% conservation (dark grey) or 60% conservation (light grey).

Table 2 Phobius transmembrane and signal sequence prediction for members of the Arabidopsis , Populus and Physcomitrella IRX10 family of proteins
Figure 2
figure 2

Phylogenetic trees for GX related proteins in Arabidopsis and Physcomitrella. Predicted protein sequences were aligned within each family, and a tree was computed using the neighbour-joining method [46] with gapped positions being excluded and branch length corrections for multiple substitutions enabled. The bars represent a PAM value (percent accepted mutations) of 10%. The numbers shown at the branch points are bootstrap values derived from 1000 randomized sequences. A) GT43 family. B) GT47 family. C) GT8 family.

The PpGT47A expression pattern indicates a role during early stages of development in physcomitrella

To investigate whether expression of PpGT47A is associated with specific tissues or developmental stages of growth, the uidA reporter gene was fused to the 3′ end of the PpGT47A gene. The construct (Figure 3A) was introduced into the Physcomitrella genome at the endogenous PpGT47A site via homologous recombination. The pattern of pGT47A expression in Physcomitrella was analysed by histochemical staining of 4 independent stable pGT47A-GUS lines, each of which showed a similar staining pattern. Expression was localised predominantly to tissues which were newly formed or undergoing expansion. Strong expression was observed in the apical region of the adult gametophore (Figure 3B), new branches forming on the side of the mature gametophore (Figure 3E) and in the tissue immediately basal to the immature sporophyte (Figure 3D). Staining was also observed in the antheridia (Figure 3C). A peak of expression was seen at the tips of the protonema side branches (Figure 3F) and the lateral buds of the chloronema (Figure 3G).

Figure 3
figure 3

The expression pattern of PpGT47A in Physcomitrella , analyzed by histochemical staining of stable pGT47A:GUS lines. (A) Schematic drawing describing the GUS construct inserted into the Physcomitrella genome. (B) Adult gametophore shows GUS staining in the apical region and in the emerging gametophore on the side of the adult gametophore. (C) GUS staining of the antheridia. (D) GUS staining in tissue below the immature sporophyte. (E) Expression peak in young gametophore growing on the side of old gametophore. (F) Protonema side branches undergoing tip growth exhibit peaks in GUS expression. (G) Bud/juvenile gametophore exhibiting GUS staining.

The PpGT47A gene partially complements the Arabidopsis irx10 irx10-Ldouble mutant

To establish whether the function of the PpGT47A enzyme is conserved between Arabidopsis and Physcomitrella, the PpGT47A gene under control of the 35S cauliflower mosaic virus (CaMV) constitutive promoter was expressed in the Arabidopsis irx10 irx10-L double mutant background. The PpGT47A gene partially rescued the irx10 irx10-L phenotype with plants forming a short inflorescence stem without the need for a protective growing cover that is normally required by the double mutant [35] (Figure 4A). Rosette diameters of complemented plants were increased by 2- to 3-fold and the inflorescence stems were between 3- and 28-fold taller compared to the irx10 irx10-L plants grown under a plastic cover (Figure 4B). Safranin staining was performed on basal stem sections of the Arabidopsis wild-type, irx10 irx10-L double mutant and complemented plants to identify regions of lignification. In Arabidopsis wild-type plants, the cell walls of the xylem vessels and interfascicular fibers were heavily stained around the whole cell (Figure 4C). In contrast, the irx10 irx10-L plants exhibited only a weak signal at the corners of the cell junctions indicating initiation of lignification, with virtually no evidence of secondary cell wall deposition in any other regions of the cell walls (Figure 4D). Irregular and variable safranin staining could be detected throughout the xylem and interfasicular fiber cell walls of stem sections from the complemented plants although the staining was less intense than in the wild-type. Despite the apparent increase in secondary cell wall production, the cell walls of irx10 irx10-L plants expressing PpGT47A were thinner than wild-type cell walls and displayed a collapsed xylem vessel phenotype (Figure 4C,D).

Figure 4
figure 4

The Physcomitrella IRX10 homolog expressed in the Arabidopsis irx10 irx10-L double mutant. A) Arabidopsis irx10 irx10-L double mutant partially complemented by p35S:PpGT47A. B) Rosette diameter and inflorescence height of PpGT47A complemented Arabidopsis plants. Data obtained from between 2 and 7 biological repeats per line. Each line represents one independent transformation event. C) Sections from 8-week old basal stem tissue of Columbia wild-type, Arabidopsis irx10 irx10-L double mutant complemented with the Physcomitrella IRX10 homolog, and the Arabidopsis irx10 irx10-L double mutant. D) Higher magnification of the safranin stained tissues shown in C. Safranin staining in the cell corners of the irx10 irx10-L double mutant is indicated by arrowheads. Scale bar 50 ÎĽm (C) or 20 ÎĽm (D).

Monosaccharide analysis was performed on cell wall material isolated from stems of the complemented plants to determine the biochemical basis for the partial complementation phenotype (Figure 5). There were no significant differences in the levels of the monosaccharides measured between the complemented lines and the irx10 irx10-L double mutant. In particular, it is noteworthy that the level of xylose remained low in the PpGT47A expressing lines in contrast to the results obtained when the Arabidopsis irx10 irx10-L double mutant was complemented with the Arabidopsis IRX10 gene [35].

Figure 5
figure 5

The PpGT47A gene does not rescue the monosaccharide composition of Arabidopsis irx10 irx10-L mutant stem tissue. A) Monosaccharide composition of stems material isolated from mature Arabidopsis wild-type plants, young wild-type plants with a 30mm stem, irx10 irx10-L double mutants and 3 independent lines of irx10 irx10-L double mutants complemented by the Physcomitrella IRX10 homolog (AtPpGT47A:16, AtPpGT47A:8, AtPpGT47A:5). Data from complemented plants are based on pooled stem material in three technical replicates for each of 3 independent biological samples pooled from multiple plants (except for samples indicated by * where only a single pooled sample was used). Data is displayed as molecular percentage of measured sugars obtained by TMS analysis from 500 ÎĽg of amylase treated AIR starting material for each sample. Error bars represent standard deviation based on three replicates.

Ppgt47AKnockout lines show no decrease in xylose or glucuronic acid content compared to wild-type

Arabidopsis irx10 and irx10-L knockout mutants have proven to be informative in elucidating the function of the encoded proteins. In order to further investigate the function of PpGT47A, Physcomitrella gt47A knockout mutants were generated. A construct was made in which the nptII coding sequence was inserted into the PpGT47A gene deleting part of exons 2 and 4 and the whole of exon 3. The construct was introduced into the Physcomitrella genome via homologous recombination resulting in the deletion of the central region of the endogenous PpGT47A gene to create a likely null knockout mutant. Knockouts were analysed by PCR using primers spanning the recombination site to identify lines in which the endogenous PpGT47A gene had been disrupted. The gametophores of the knockout lines were visually similar to wild-type with no obvious morphological changes when grown on BCD media (Additional file 1: Figure S1). Further experiments were carried out to test whether varying the composition of the growth media by addition of different sugars or hormones under different light conditions (see materials and methods for details) revealed any phenotypic changes in the knockout lines but none were observed (data not shown). Monosaccharide analysis of gametophore cell walls from the knockout lines (Figure 6) did not show any significant differences compared to the wild-type. Of particular interest is the observation that there was no difference in xylose content between knockout and wild-type gametophores in contrast to the results obtained for the Arabidopsis irx10 and irx10-L mutants [35].

Figure 6
figure 6

Knockout of the Physcomitrella PpGT47A gene does not cause a significant change in cell wall monosaccharide composition. A) Schematic drawing of the PpGT47A gene and the knock-out construct which was introduced via homologous recombination to obtain knockout mutants in Physcomitrella. ** corresponds to a truncated version of the E4 sequence and * corresponds to a truncated version of the 3′UTR sequence which are indicated in the upper genomic sequence. B) Monosaccharide analysis of gametophore cell walls from Physcomitrella wild-type and 4 independent gt47a knockout mutants. Data were obtained from 3 technical replicates of two pooled samples for the wild-type and knockout Ppgt47a:3, and three pooled samples for knockouts Ppgt47a:2; Ppgt47a:5 and Ppgt47a:11.

Discussion

An important developmental adaptation of land plants involved the ability to form conductive tissues allowing efficient exploitation of available mineral and water resources. It has been suggested that the xylan polymer could have provided a pre-adaptive advantage to ancestors of vascular plants and contributed to the evolution of efficient water conducting systems [47]. Detection of glucuronoxylan in Physcomitrella[9, 12] shows that the xylan polymer was present in a common ancestor prior to divergence of the bryophytes and vascular plants. The finding that the Physcomitrella PpGT47A gene is able to partially substitute for the lack of function of IRX10 or IRX10-L in Arabidopsis together with the high degree of sequence conservation further strengthens the argument that there was a common ancestor protein. Despite this, components of the GX synthesis machinery appear to have evolved with the result that the Arabidopsis IRX10, IRX10-L and the Physcomitrella GT47A proteins although apparently originating from a common ancestor, do not exhibit identical functions or activities.

It has been speculated that the Arabidopsis IRX10 protein forms a complex together with AtIRX9 and AtIRX14 and that this complex is responsible for the synthesis of the backbone of GX [39, 40]. AtGUX1 and AtGUX2 are proposed to add the GlcA side chains to the backbone [38] while IRX8, FRA8 and PARVUS are thought to synthesise the reducing end oligosaccharide [19, 29, 31, 32, 40]. Interestingly, Physcomitrella homologs can be identified for all of the known GX synthesis proteins with the exception of IRX8 and PARVUS. Recent studies suggests that xylan structure in Physcomitrella differs from that of higher plants and may as in the grasses lack the reducing end oligosaccharide which otherwise is thought to be universally conserved amongst the dicots. The ability to synthesise the reducing end oligosaccharide structure thus may be a relatively recent adaptation that is only found in some higher plants.

A previous study utilised a number of anti-xylan antibodies which recognise distinct epitopes to localise xylan in Physcomitrella[12]. These antibodies produced different labelling patterns – for example LM11 which strongly labels axillary hair cells and CCRC-M137 which shows labelling of leaf cell walls in addition to the axillary hair cells. In this study, the Physcomitrella IRX10 promoter was found to direct expression of the GUS reporter in the apical region of the adult gametophore, new branches forming from the gametophore and tissues basal to the immature sporophyte (Figure 3). There was no preferential staining of axillary hairs observed in any of the GUS lined studied. However, the antibody recognition of xylan in axillary hairs does not rule out presence of xylan epitopes masked by other cell wall components in other Physcomitrella cell wall tissues. Furthermore, the possibility that PpIRX10 functions in making a different polysaccharide or makes a form of xylan in Physcomitrella which is not recognised by the currently available anti-xylan antibodies cannot be discounted. In the absence of a functional enzymatic assay for PpIRX10 it is currently not possible to be certain about its enzymatic activity, although it is reasonable to hypothesise that it plays a role in xylan biosynthesis, a conclusion which is supported by the partial complementation of the Arabidopsis irx10 irx10-L double mutant.

Failure of PpGT47A to fully complement the irx10 irx10-L Arabidopsis mutant supports functional divergence between the Arabidopsis and physcomitrellaIRX10 family of proteins

The finding that the Physcomitrella GT47A protein only partially rescues the Atirx10 irx10-L double mutant demonstrates that although the proteins are highly conserved at the sequence level, there are important differences which influence function. There are a number of possible reasons for these apparent functional differences. Firstly, the enzymatic activity of PpGT47A may be different to that of the Arabidopsis IRX10 or IRX10-L proteins. Despite the high degree of sequence conservation between the Arabidopsis and Physcomitrella IRX10 proteins, subtle amino acid differences could give an altered enzymatic activity but in the absence of a functional enzymatic assay this cannot currently be tested. Alternatively, PpGT47A could have the same enzymatic activity as the Arabidopsis IRX10 but the interaction between IRX9 and/or IRX14 to form a putative functional complex may not be optimal. A third possibility is that the targeting or subcellular localisation of PpGT47A is not correct when expressed in Arabidopsis. The highly divergent N-terminal domain that in the Arabidopsis IRX10 protein encodes a predicted signal peptide, in Physcomitrella instead forms a predicted transmembrane domain (Table 2). Thus, mislocalisation and/or a different conformation of the PpGT47A protein compared to AtIRX10 may combine to produce only a small amount of a functional GX synthesis complex or alternatively a complex with low activity in the partially complemented Arabidopsis plants.

Evolutionary adaption of the IRX10 family of enzymes

The Arabidopsis IRX10 and Populus PtGT47A-1 genes are expressed within the vascular tissue made up mainly of cells rich in secondary cell walls. Bryophyte water conducting tissues in contrast do not form thickened cell walls and so it is unsurprising that the expression pattern of PpGT47A differs from that of the Arabidopsis homologs. The ability of PpGT47A to partially complement the Arabidopsis irx10 irx10-L double mutant plants shows that there is a degree of functional overlap between the Arabidopsis and Physcomitrella enzymes but that either activity, conformation or targeting of the enzymes prevent full rescue of the wild-type phenotype. Interestingly, the degree of similarity is higher between PpGT47A and AtIRX10-L than for AtIRX10 indicating that IRX10-L is closer to the ancestral form of the protein. The expression of PpGT47A in Physcomitrella tissues undergoing primary cell wall formation contrasts with that of the Arabidopsis IRX10 gene which is associated with tissues forming secondary cell walls. In vascular plants, the IRX10 family appears to have undergone a sub- or neo-functionalisation resulting in at least a subset of the genes becoming specialised for secondary cell wall formation.

Analysis of the monosaccharide sugar composition of cell walls isolated from the irx10 irx10-L lines partially complemented with the PpGT47A gene does not show any significant changes in comparison to the irx10 irx10-L double mutant indicating that either changes are in a minor component of the cell wall and thus below the detection limit or that the PpGT47A function is not related to the cell wall composition. Although current evidence strongly indicates that IRX10 and related proteins from other plants function in glucuronoxylan biosynthesis, there have been previous reports suggesting involvement of the tobacco NpGUT1, another member of the IRX10 family of proteins, in rhamnogalacturonan II (RGII) biosynthesis, adding GlcA to one of the side chains of the RGII polysaccharide [48]. The decrease in the level of GlcA reported for the Npgut1 tobacco mutant is greater than can be explained by a reduction in RGII levels alone arguing against NpGUT1 having a sole function in RGII synthesis. Interestingly, the Npgut1 mutant also exhibits a decrease in xylose content, implying that xylan synthesis could also be affected. Furthermore, the tobacco NpGUT1 protein is able to perform the same enzymatic function as the Arabidopsis IRX10, restoring xylan levels to those of the wild-type when fused with the N-terminal 71 amino acid domain of the AtIRX10 protein and expressed in the irx10 irx10-L background [35]. Although this result supports an involvement of NpGUT1 in glucuronoxylan biosynthesis, the possibility that members of the IRX10 family, including PpGT47A, could function in the synthesis of RGII or an RGII-like polymer cannot currently be discounted.

The role of PpGT47A in physcomitrella

A major advantage of using Physcomitrella is the possibility to make clean loss of function mutants by homologous recombination. This approach was used to create a knockout mutant for the PpGT47A gene. However, the knockout mutant had no obvious phenotypes under the conditions tested, nor did monosaccharide analysis of the gametophore cell wall reveal any significant changes in the mutant (Figure 6). We conclude from this that loss of PpGT47A function either does not affect the cell wall composition, or alternatively that any such effects are too subtle to be detected in our analysis. It should be noted that RGII and xylan are both known to be minor components of the bryophyte cell wall [9, 10], and alterations in the composition of either or both polymers might therefore have escaped detection in our analysis of total cell wall material.

The absence of an obvious knockout phenotype could be due to several reasons. It is possible that the PpGT47A gene is functionally duplicated in Physcomitrella. Although this is unlikely since there are no close homologues of PpGT47A in the Physcomitrella genome [49], the possibility exists that another more distantly related GT can provide the same function as PpGT47A. Alternatively, it is possible that the modifications catalyzed by PpGT47A are important in Physcomitrella only under certain conditions, such as abiotic stress, but not under standard laboratory conditions. In any case, the fact that PpGT47A is strongly conserved and shows no evidence of being a pseudogene suggests that it encodes a functional protein, a conclusion that is reinforced by its ability to partially complement the Arabidopsis irx10 irx10-L double mutant.

Conclusions

Genes encoding the enzymes required for synthesis of the GX backbone are highly conserved between Physcomitrella, Arabidopsis and Populus highlighting the importance of the polysaccharide throughout the plant kingdom. While the precise function of the Physcomitrella GT47A gene remains to be elucidated, its ability to partially complement the Arabidopsis irx10 irx10-L double mutant demonstrates that it encodes a GT with similar functional specificity to AtIRX10 and AtIRX10-L. Interestingly the absence of homologs of IRX8 and PARVUS in the Physcomitrella genome indicates that the ability to synthesise the reducing end oligosaccharide of GX is an adaptation only found in higher plants. It is tempting to speculate that evolution of the GX biosynthesis machinery may have been a key step in the evolution of higher plants.

Methods

Bioinformatics

The Physcomitrella patens subsp patens v1.1 database and the Phytozome Physcomitrella database (http://www.phytozome.net/physcomitrella.php) were used to search for homologs using the Arabidopsis IRX10, IRX10-L, IRX9, IRX9-L, IRX14, IRX14-L, IRX8, PARVUS, GUX1 and GUX2 proteins. Sequences were aligned using Clustal-W software. Phylogenetic trees (Figure 2) were computed using the neighbour-joining method [46] as implemented in the Clustal-X software. The Phobius signal peptide and transmembrane prediction software was used for topological analysis (phobius.sbc.su.se) [44, 47].

Growth conditions

Arabidopsis was grown under long day conditions (16h light/8h dark) at a maximum irradiation of 150 μmolm-2s-1, 60% humidity with 22°C day and 18°C night temperatures. Physcomitrella gametophores were grown on BCD media (0.001 M MgSO4, 0.0189 mM KH2PO4, 0.01 M KNO3, 0.045 mM FeSO4, alternative trace element solution (TES) as described on http://moss.nibb.ac.jp/) and protonemata tissues were grown on MM media (BCD media with 5mM ammonium tartrate). Light, humidity, and temperature conditions employed were as for Arabidopsis.

Overexpression and knock-out constructs

PpGT47A was PCR amplified from Physcomitrella DNA using forward primer (F): 5′-ggggacaagtttgtacaaaaaagcaggctgggagaattgggtgtttcg-3′ and reverse primer (R): 5′-ggggaccactttgtacaagaaagctgggtgtgttacaaatcattgcccc-3′), cloned into pDONR207 and then transferred into the pEarleyGate 100 destination vector [50] using the Gateway cloning system. The PpGT47A overexpression construct was introduced into the Arabidopsis irx10 irx10-L(+/-) background [36] using the floral dip method [51]. Transformed lines were screened using BASTA (Hoechst Schering AgrEvo GmbH, Germany) selection and irx10 irx10-L double mutants identified by PCR [35] allowing lines containing the transgene in a homozygous irx10 irx10-L background to be selected in the T2 generation. Wild-type and transformed mutant seed were sown and treated as previously described [35].

To generate the PpGT47A knock-out construct, the NptII gene was PCR amplified from the pMT164 vector, introducing an XmaI restriction site (F: 5′-aattcccggggagtcaaag-3′ and R: 5′-atggatcgatgttaacatgc-3′). PpGT47A was PCR amplified from Physcomitrella Gransden 2004 (F: 5′-ggacatagaagcatgatgc-3′ and R: 5′-ggaatacaacacgattcc-3′) and cloned into TOPO2.1 vector. The TOPO2.1 vector containing the PpGT47A gene was cut by XmaI and MfeI, the NptII cassette was cut with XmaI and EcoRI, and the two DNA fragments ligated using T4 DNA-ligase. The resulting construct was linearized by EcoRI before being transformed into Gransden 2004 wild-type protoplasts [52] using PEG mediated transformation as described previously [53]. Stable transformants were identified by selection on kanamycin-containing media for 2 weeks, followed by growth on selection free media for 2 weeks and then a further hygromycin selection for 2 weeks. Transformants were confirmed by PCRs spanning the recombination sites. Primers used for verification of the knockout construct were F1: tggtcaggagaatcatgc and F2: cggaagtaacagaatgagg, R1 ttgataactgtgggttacc and R2: caggtgacatgagactcg, and for the insert F: ttcgctcatgtgttgagc and R: aggcatcttcaacgatgg. All restriction enzymes used were FastDigest, Fermentas (St. Leon Rot, Germany).

GUS construct

The GUS reporter gene was fused to the PpGT47A gene in the Physcomitrella genome using the following strategy. Two fragments, one homologous to the DNA sequence upstream and one to the region downstream of the PpGT47A stop codon, were amplified from endogenous Physcomitrella Gransden 2004 DNA by PCR. The PCR for the upstream fragment introduced a BamHI and a XbaI site at the 5′ end with the forward primer and the stop codon was disrupted with the reverse primer (F: 5′-ggatccttctttctagtgacaatcgg-3′ and R: 5′-cgcggatccacaaatcattgccccaagg-3′). The downstream fragment was amplified using F: 5′-ctttcttggaatactcacc-3 and R: 5′-ctggaacgcatctagacc-3′ primers. The fragments were cloned separately into the Topo2.1 vector. The cloned downstream fragment was excised with NotI and XbaI and ligated into a modified Topo vector carrying the GUS gene [54]. The upstream PCR fragment was cut with BamHI and introduced into Topo vector carrying the downstream fragment and the GUS gene. All restriction enzymes were FastDigest, Fermentas.

GUS staining

The composition of the BCD media and the growth conditions in the light chamber were as previously described [45]. Clumps of subcultured protonema tissue were placed on BCD plates and grown for three weeks in continuous light at 25°C and then moved to short day conditions (8 hours light/16 hours dark at 15°C) and grown for three months. GUS staining was performed by incubating the moss tissue in X-gluc substrate solution as described by the Physcobase protocol (http://moss.nibb.ac.jp/). Stained tissue was analyzed with an Olympus SZX12 stereo microscope and images recorded using an Olympus XC30 camera.

Phenotyping of Ppgt47Aknockout lines

Small clumps of subcultured protonema tissue (approximately 2 mm in diameter) were used to inoculate standard BCD plates and plates containing different additions. The additions were 0.15 M glucose, 0.15 M fructose, 0.15M sucrose, 0.15 M mannitol or 5 mM ammonium tartrate. The plates were placed vertically in an incubator under three different conditions, high light (30 ÎĽmol/m2s), low light (6 ÎĽmol/m2s) or complete darkness. In addition, morphology studies were carried out on Physcomitrella grown on BCD plates containing the following conditions and concentrations of hormones. High light: 7 ÎĽM BAP, 1 ÎĽM ABA, 0.5 ÎĽM IAA and 10 ÎĽM GA3. Low light: 0.5 ÎĽM BAP, 0.5 ÎĽM ABA, 0.5 ÎĽM IAA and 10 ÎĽM GA3. All hormones were from Sigma Aldrich (Stockholm, Sweden). Plates were observed for two months.

Sugar analysis

Basal stem regions from wild-type Arabidopsis plants measuring 30 mm in height or 6 weeks old, 9-week old mutant or complemented plants and 8-week old Physcomitrella gametophores grown on BCD media were used for monosaccharide analysis. Tissues were collected in 80% ethanol and stored at -80°C until being freeze dried (Modulyo, Edwards, West Sussex, UK). Dried material was ball milled in a beadmill (Retsch MM301, Haan, Germany) for 2×30s at 30 Hz. Alcohol insoluble residues (AIR) were obtained as previously described [39]. The AIR material was suspended in 0.1 M phosphate buffer, pH7 containing 0.01% sodium azide. Alpha-amylase (Roche, Indianapolis, USA) was added at a concentration of 1000U per 1g of cell wall material and the material was digested with gentle shaking for 24h at 37°C. The procedure was repeated once before the pellet was washed first with 0.1 M phosphate buffer pH 7, then with water and finally acetone. The material obtained was analysed using the TMS method [55–57].

Tissue sections

Basal stem segments were collected, fixed in FAA (5% Acetic acid, 50% ethanol, 5% formadehyde in dH2O) and stored at 4°C until being sectioned using a vibratome (60 μm thickness) (Leica VT1000S, Germany), stained with 1:2 filtered safranin (1% in 50% ethanol): alcian blue (1% in H20, 1% formalin and 0.15% glacial acetic acid), rinsed in H2O and mounted in 50% glycerol [58].

Abbreviations

GT:

Glycosyltransferase

AGP:

Arabinogalactan protein

GX:

Glucuronoxylan

IRX:

Irregular xylem

CaMV:

Cauliflower Mosaic Virus

GlcA:

Glucuronic acid

GA3:

Gibberellic acid

ABA:

Abscisic acid

BAP:

6-benzylamino purine

IAA:

Indole-3-acetic acid

AIR:

Alcohol insoluble residues.

References

  1. Popper ZA, Tuohy MG: Beyond the green: understanding the evolutionary puzzle of plant and algal cell walls. Plant Physiol. 2010, 153: 373-383. 10.1104/pp.110.158055.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  2. Popper ZA, Michel G, Herve C, Domozych DS, Willats WGT, Tuohy MG, Kloareg B, Stengel DB: Evolution and diversity of plant cell walls: from algae to flowering plants. Ann Rev Plant Biol. 2011, 62: 567-588. 10.1146/annurev-arplant-042110-103809.

    Article  CAS  Google Scholar 

  3. Sørensen I, Pettolino FA, Bacic A, Ralph J, Lu F, O’Neill MA, Fei Z, Rose JKC, Domozych DS, Willats WGT: The charophycean green algae provide insights into the early origins of plant cell walls. Plant J. 2011, 68: 201-211. 10.1111/j.1365-313X.2011.04686.x.

    Article  PubMed  Google Scholar 

  4. Brown RM: Cellulose microfibril assembly and orientation - recent developments. J Cell Sci. 1985, 2: 13-32.

    Article  Google Scholar 

  5. Ligrone R, Vaughn KC, Renzaglia KS, Knox JP, Duckett JG: Diversity in the distribution of polysaccharide and glycoprotein epitopes in the cell walls of bryophytes: new evidence for the multiple evolution of water-conducting cells. New Phytol. 2002, 156: 491-508. 10.1046/j.1469-8137.2002.00538.x.

    Article  CAS  Google Scholar 

  6. Popper ZA, Fry SC: Primary cell wall composition of bryophytes and charophytes. Ann Bot. 2003, 91: 1-12. 10.1093/aob/mcg013.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  7. Kremer C, Pettolino F, Bacic A, Drinnan A: Distribution of cell wall components in sphagnum hyaline cells and in liverwort and hornwort elaters. Planta. 2004, 219: 1023-1035. 10.1007/s00425-004-1308-4.

    Article  PubMed  CAS  Google Scholar 

  8. Lee KJD, Sakata Y, Mau SL, Pettolino F, Bacic A, Quatrano RS, Knight CD, Knox JP: Arabinogalactan proteins are required for apical cell extension in the moss physcomitrella patens. Plant Cell. 2005, 17: 3051-3065. 10.1105/tpc.105.034413.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  9. Moller I, Sorensen I, Bernal AJ, Blaukopf C, Lee K, Obro J, Pettolino F, Roberts A, Mikkelsen JD, Knox JP, Bacic A, Willats WG: High-throughput mapping of cell-wall polymers within and between plants using novel microarrays. Plant J. 2007, 50: 1118-1128. 10.1111/j.1365-313X.2007.03114.x.

    Article  PubMed  CAS  Google Scholar 

  10. Matsunaga T, Ishii T, Matsumoto S, Higuchi M, Darvill A, Albersheim P, O’Neill MA: Occurrence of the primary cell wall polysaccharide rhamnogalacturonan II in pteridophytes, lycophytes, and bryophytes. Implications for the evolution of vascular plants. Plant Physiol. 2002, 134: 339-351.

    Article  Google Scholar 

  11. Peña MJ, Darvill AG, Eberhard S, York WS, O’Neill MA: Moss and liverwort xyloglucans contain galacturonic acid and are structurally distinct from the xyloglucans synthesized by hornworts and vascular plants. Glycobiology. 2008, 18: 891-904. 10.1093/glycob/cwn078.

    Article  PubMed  Google Scholar 

  12. Kulkarni AR, Peña MJ, Acvi U, Mazumder K, Urbanowicz BR, Pattathil S, Yin Y, O’Neill MA, Roberts A, Hahn MG, Xu Y, Darvill AG, York WS: The ability of land plants to synthesize glucuronoxylans predates the evolution of tracheophytes. Glycobiology. 2012, 22: 439-451. 10.1093/glycob/cwr117.

    Article  PubMed  CAS  Google Scholar 

  13. Carafa A, Duckett JG, Knox JP, Ligrone R: Distribution of cell-wall xylans in bryophytes and tracheophytes: new insights into basal interrelationships of land plants. New Phytol. 2005, 168: 231-240. 10.1111/j.1469-8137.2005.01483.x.

    Article  PubMed  CAS  Google Scholar 

  14. Teleman A, Lundqvist J, Tjerneld F, Stalbrand H, Dahlman O: Characterization of acetylated 4-O-methylglucuronoxylan isolated from aspen employing H-1 and C-13 NMR spectroscopy. Carbohydrate Res. 2000, 329: 807-815. 10.1016/S0008-6215(00)00249-4.

    Article  CAS  Google Scholar 

  15. Decou R, Lhernould S, Laurans F, Sulpice E, Leple JC, Dejardin A, Pilate G, Costa G: Cloning and expression analysis of a wood-associated xylosidase gene (PtaBXL1) in poplar tension wood. Phytochemistry. 2009, 70: 163-172. 10.1016/j.phytochem.2008.12.019.

    Article  PubMed  CAS  Google Scholar 

  16. Zhou GK, Zhong RQ, Richardson EA, Morrison WH, Nairn CJ, Wood-Jones A, Ye ZH: The poplar glycosyltransferase GT47C is functionally conserved with Arabidopsis fragile Fiber8. Plant Cell Physiol. 2006, 47: 1229-1240. 10.1093/pcp/pcj093.

    Article  PubMed  CAS  Google Scholar 

  17. Zhou GK, Zhong R, Himmelsbach DS, McPhail BT, Ye ZH: Molecular characterization of PoGT8D and PoGT43B, Two secondary wall-associated glycosyltransferases in poplar. Plant Cell Physiol. 2007, 48: 689-699. 10.1093/pcp/pcm037.

    Article  PubMed  CAS  Google Scholar 

  18. Lee C, Teng Q, Huang WL, Zhong RQ, Ye ZH: The poplar GT8E and GT8F glycosyltransferases are functional orthologs of Arabidopsis PARVUS involved in glucuronoxylan biosynthesis. Plant Cell Physiol. 2009, 50: 1982-1987. 10.1093/pcp/pcp131.

    Article  PubMed  CAS  Google Scholar 

  19. Lee CH, Zhong RQ, Richardson EA, Himmelsbach DS, McPhail BT, Ye ZH: The PARVUS gene is expressed in cells undergoing secondary wall thickening and is essential for glucuronoxylan biosynthesis. Plant Cell Physiol. 2007, 48: 1659-1672. 10.1093/pcp/pcm155.

    Article  PubMed  CAS  Google Scholar 

  20. Lee CH, Teng Q, Huang WL, Zhong RQ, Ye ZH: Down-regulation of PoGT47C expression in poplar results in a reduced glucuronoxylan content and an increased wood digestibility by cellulase. Plant Cell Physiol. 2009, 50: 1075-1089. 10.1093/pcp/pcp060.

    Article  PubMed  CAS  Google Scholar 

  21. Lee C, Teng Q, Zhong R, Ye ZH: Molecular dissection of xylan biosynthesis during wood formation in poplar. Mol Plant. 2011, 4: 730-747. 10.1093/mp/ssr035.

    Article  PubMed  CAS  Google Scholar 

  22. Li Q, Min D, Wang JPY, Peszlen I, Horvath L, Horvath B, Nishimura Y, Jameel H, Chang HM, Chiang VL: Down-regulation of glycosyltransferase 8D genes in populus trichocarpa caused reduced mechanical strength and xylan content in wood. Tree Physiol. 2011, 31: 226-236. 10.1093/treephys/tpr008.

    Article  PubMed  CAS  Google Scholar 

  23. Ebringerova A, Heinze T: Xylan and xylan derivatives - biopolymers with valuable properties, 1 - naturally occurring xylans structures, procedures and properties. Macromol Rapid Comm. 2000, 21: 542-556. 10.1002/1521-3927(20000601)21:9<542::AID-MARC542>3.0.CO;2-7.

    Article  CAS  Google Scholar 

  24. Shimizu K, Ishihara M, Ishihara T: Hemicellulases of brown rotting fungus tyromyces palustris. II. The oligosaccharides from the hydrolysate of a hardwood xylan by the intracellular xylanase. Mokuzai Gakkaishi (J Japan Wood Res Soc). 1976, 22: 618-625.

    CAS  Google Scholar 

  25. Johansson MH, Samuelson O: Reducing end groups in birch xylan and their alkaline-degradation. Wood Sci Tech. 1977, 11: 251-263. 10.1007/BF00356924.

    Article  CAS  Google Scholar 

  26. Aspinall GO: Chemistry of cell wall polysaccharides. The biochemistry of plants: a comprehensive treatise. Vol. 3rd edition. Edited by: Stumpf PK, Conn EE. Academic Press, New York; 1990: 473-500.

    Google Scholar 

  27. Aspinall GO: Chemistry of cell wall polysaccharides. Biochemistry of plants. A comprehensive treatise. Vol. 3rd edition. Edited by: Stumpf CPK, Conn EE. Academic Press, New York; 1980: 473-500.

    Google Scholar 

  28. Andersson SI, Samuelson O, Ishihara M, Shimizu K: Structure of the reducing end-groups in spruce xylan. Carbohydrate Res. 1983, 111: 283-288. 10.1016/0008-6215(83)88312-8.

    Article  CAS  Google Scholar 

  29. Zhong RQ, Peña MJ, Zhou GK, Nairn CJ, Wood-Jones A, Richardson EA, Morrison WH, Darvill AG, York WS, Ye ZH: Arabidopsis fragile fiber8, which encodes a putative glucuronyltransferase, is essential for normal secondary wall synthesis. Plant Cell. 2005, 17: 3390-3408. 10.1105/tpc.105.035501.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  30. Lee CH, O’Neill MA, Tsumuraya Y, Darvill AG, Ye ZH: The irregular xylem9 mutant is deficient in xylan xylosyltransferase activity. Plant Cell Physiol. 2007, 48: 1624-1634. 10.1093/pcp/pcm135.

    Article  PubMed  CAS  Google Scholar 

  31. Peña MJ, Zhong R, Zhou GK, Richardson EA, O’Neill MA, Darvill AG, York WS, Ye ZH: Arabidopsis irregular xylem8 and irregular xylem9: implications for the complexity of glucuronoxylan biosynthesis. Plant Cell. 2007, 19: 549-563. 10.1105/tpc.106.049320.

    Article  PubMed  PubMed Central  Google Scholar 

  32. Persson S, Caffall KH, Freshour G, Hilley MT, Bauer S, Poindexter P, Hahn MG, Mohnen D, Somerville C: The Arabidopsis irregular xylem8 mutant is deficient in glucuronoxylan and homogalacturonan, which are essential for secondary cell wall integrity. Plant Cell. 2007, 19: 237-255. 10.1105/tpc.106.047720.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  33. Brown DM, Zhang ZN, Stephens E, Dupree P, Turner SR: Characterization of IRX10 and IRX10-like reveals an essential role in glucuronoxylan biosynthesis in Arabidopsis. Plant J. 2009, 57: 732-746. 10.1111/j.1365-313X.2008.03729.x.

    Article  PubMed  CAS  Google Scholar 

  34. Lee CH, Teng Q, Huang WL, Zhong RQ, Ye ZH: The F8H glycosyltransferase is a functional paralog of FRA8 involved in glucuronoxylan biosynthesis in Arabidopsis. Plant Cell Physiol. 2009, 50: 812-827. 10.1093/pcp/pcp025.

    Article  PubMed  CAS  Google Scholar 

  35. Wu AM, Rihouey C, Seveno M, Hornblad E, Singh SK, Matsunaga T, Ishii T, Lerouge P, Marchant A: The Arabidopsis IRX10 and IRX10-LIKE glycosyltransferases are critical for glucuronoxylan biosynthesis during secondary cell wall formation. Plant J. 2009, 57: 718-731. 10.1111/j.1365-313X.2008.03724.x.

    Article  PubMed  CAS  Google Scholar 

  36. Keppler BD, Showalter AM: IRX14 And IRX14-LIKE, Two glycosyl transferases involved in glucuronoxylan biosynthesis and drought tolerance in Arabidopsis. Mol Plant. 2010, 3: 834-841. 10.1093/mp/ssq028.

    Article  PubMed  CAS  Google Scholar 

  37. Lee C, Teng Q, Huang WL, Zhong RQ, Ye ZH: The Arabidopsis family GT43 glycosyltransferases form two functionally nonredundant groups essential for the elongation of glucuronoxylan backbone. Plant Physiol. 2010, 153: 526-541. 10.1104/pp.110.155309.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  38. Mortimer JC, Miles GP, Brown DM, Zhang ZN, Segura MP, Weimar T, Yu XL, Seffen KA, Stephens E, Turner SR, Dupree P: Absence of branches from xylan in Arabidopsis gux mutants reveals potential for simplification of lignocellulosic biomass. Proc Natl Acad Sci USA. 2010, 107: 17409-17414. 10.1073/pnas.1005456107.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  39. Wu AM, Hornblad E, Voxeur A, Gerber L, Rihouey C, Lerouge P, Marchant A: 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. 2010, 153: 542-554. 10.1104/pp.110.154971.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  40. Brown DM, Goubet F, Vicky WWA, Goodacre R, Stephens E, Dupree P, Turner SR: Comparison of five xylan synthesis mutants reveals new insight into the mechanisms of xylan synthesis. Plant J. 2007, 52: 1154-1168. 10.1111/j.1365-313X.2007.03307.x.

    Article  PubMed  CAS  Google Scholar 

  41. Lee C, Zhong R, Ye ZH: Arabidopsis family GT43 members are xylan xylosyltransferases required for the elongation of the xylan backbone. Plant Cell Physiol. 2012, 53: 135-143. 10.1093/pcp/pcr158.

    Article  PubMed  Google Scholar 

  42. Kong YZ, Zhou GK, Avci U, Gu XG, Jones C, Yin YB, Xu Y, Hahn MG: Two poplar glycosyltransferase genes, PdGATL1.1 And PdGATL1.2, are functional orthologs to PARVUS/AtGATL1 in Arabidopsis. Mol Plant. 2009, 2: 1040-1050. 10.1093/mp/ssp068.

    Article  PubMed  CAS  Google Scholar 

  43. Käll L, Krogh A, Sonnhammer ELL: A combined transmembrane topology and signal peptide prediction method. J Mol Biol. 2004, 338: 1027-1036. 10.1016/j.jmb.2004.03.016.

    Article  PubMed  Google Scholar 

  44. Käll L, Krogh A, Sonnhammer ELL: Advantages of combined transmembrane topology and signal peptide prediction - the phobius web server. Nucleic Acids Res. 2007, 35: W429-W432. 10.1093/nar/gkm256.

    Article  PubMed  PubMed Central  Google Scholar 

  45. Nilsson A, Olsson T, Ulfsted M, Thelander M, Ronne H: Two novel types of hexokinases in the moss physcomitrella patens. BMC Plant Biol. 2011, 11: 32. 10.1186/1471-2229-11-32.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  46. Saitou N, Nei M: The neighbor-joining method: a new method for reconstructing phylogenetic trees. Mol Biol Evol. 1987, 4: 406-425.

    PubMed  CAS  Google Scholar 

  47. Popper ZA: Evolution and diversity of green plant cell walls. Current Opinion Plant Biol. 2008, 11: 286-292. 10.1016/j.pbi.2008.02.012.

    Article  CAS  Google Scholar 

  48. Iwai H, Masaoka N, Ishii T, Satoh S: A pectin glucuronyltransferase gene is essential for intercellular attachment in the plant meristem. Proc Nat Acad Sci USA. 2002, 99: 16319-16324. 10.1073/pnas.252530499.

    Article  PubMed  CAS  PubMed Central  Google Scholar 

  49. Scheller HV, Ulvskov P: Hemicelluloses. Ann Rev Plant Biol. 2010, 61: 263-289. 10.1146/annurev-arplant-042809-112315.

    Article  CAS  Google Scholar 

  50. Earley KW, Haag JR, Pontes O, Opper K, Juehne T, Song KM, Pikaard CS: Gateway-compatible vectors for plant functional genomics and proteomics. Plant J. 2006, 45: 616-629. 10.1111/j.1365-313X.2005.02617.x.

    Article  PubMed  CAS  Google Scholar 

  51. Clough SJ, Bent AF: Floral dip: a simplified method for agrobacterium-mediated transformation of Arabidopsis thaliana. Plant J. 1998, 16: 735-743. 10.1046/j.1365-313x.1998.00343.x.

    Article  PubMed  CAS  Google Scholar 

  52. Cove D: The moss physcomitrella patens. Ann Rev Genetics. 2005, 39: 339-358. 10.1146/annurev.genet.39.073003.110214.

    Article  CAS  Google Scholar 

  53. Schaefer D, Zryd JP, Knight CD, Cove DJ: Stable transformation of the moss physcomitrella patens. Mol Gen Genet. 1991, 226: 418-424.

    Article  PubMed  CAS  Google Scholar 

  54. Eklund DM, Thelander M, Landberg K, Staldal V, Nilsson A, Johansson M, Valsecchi I, Pederson ERA, Kowalczyk M, Ljung K, Ronne H, Sundberg E: Homologues of the Arabidopsis thaliana SHI/STY/LRP1 genes control auxin biosynthesis and affect growth and development in the moss physcomitrella patens. Development. 2010, 137: 1275-1284. 10.1242/dev.039594.

    Article  PubMed  CAS  Google Scholar 

  55. Sweely CC, Bentley R, Makita M, Wells WW: Gas-liquid chromatography of trimethylsilyl derivatives of sugars and related substances. J American Chem Soc. 1963, 85: 2497-2507. 10.1021/ja00899a032.

    Article  Google Scholar 

  56. Englyst HN, Cummings JH: Simpified method for the measurement of total non-starch polysaccharides by gas- liquid-chromatography of constituent sugars as alditol acetates. Analyst. 1984, 109: 937-942. 10.1039/an9840900937.

    Article  CAS  Google Scholar 

  57. Harholt J, Jensen JK, Sorensen SO, Orfila C, Pauly M, Scheller HV: ARABINAN DEFICIENT 1 is a putative arabinosyltransferase involved in biosynthesis of pectic arabinan in Arabidopsis. Plant Phys. 2006, 140: 49-58.

    Article  CAS  Google Scholar 

  58. Srebotnik E, Messner K: A simple method that uses differential staining and light-microscopy to assess the selectivity of wood delignification by white-rot fungi. App Environ Microbiol. 1994, 60: 1383-1386.

    CAS  Google Scholar 

Download references

Acknowledgements

We acknowledge help from the group of Ewa Mellerowicz in measuring MeGlc using an unpublished protocol. Junko Schmidt provided support in running the MS analysis of monosaccharides.

Urs Fischer, Björn Sundberg, Christine Ratke and Benjamin Bollhöner are thanked for helpful critical reading of a previous version of this work produced by Emma Hörnblad for her PhD thesis. Magnus Eklund provided the modified TOPO vector used in making the GUS construct.

This work was supported by grant 621-2011-6004 from the Swedish Research Council VR (HR) and the Formas FuncFiber Center of Excellence (http://www.funcfiber.se) (AM, EH).

Author information

Authors and Affiliations

Authors

Corresponding author

Correspondence to Alan Marchant.

Additional information

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

EH carried out the bioinformatics, complementation experiments, cell wall analysis, generated all constructs and wrote the majority of the paper. MU performed the moss transformations, analysis of knockout phenotypes and GUS histochemistry. HR was involved in discussions, bioinformatics, writing the manuscript and provided facilities. AM conceived and supervised the project, and was involved in writing the paper. All authors read and approved the final manuscript.

Electronic supplementary material

12870_2012_1187_MOESM1_ESM.pdf

Additional file 1 Figure S1.: Physcomitrella patens wild-type colony and Ppgt47a knock out colony. The plants were grown for 6 weeks on BCD media supplemented with 5 mM ammonium tartrate. A. Wild-type. B. Ppgt47a. (PDF 172 KB)

Authors’ original submitted files for images

Rights and permissions

Open Access This article is published under license to BioMed Central Ltd. This is an Open Access article is distributed under the terms of the Creative Commons Attribution License ( https://creativecommons.org/licenses/by/2.0 ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Reprints and permissions

About this article

Cite this article

Hörnblad, E., Ulfstedt, M., Ronne, H. et al. Partial functional conservation of IRX10 homologs in physcomitrella patens and Arabidopsis thalianaindicates an evolutionary step contributing to vascular formation in land plants. BMC Plant Biol 13, 3 (2013). https://doi.org/10.1186/1471-2229-13-3

Download citation

  • Received:

  • Accepted:

  • Published:

  • DOI: https://doi.org/10.1186/1471-2229-13-3

Keywords