The Arabidopsis Class III Peroxidase AtPRX71 Negatively Regulates Growth under Physiological Conditions and in Response to Cell Wall Damage  

Abstract

The structure of the cell wall has a major impact on plant growth and development, and alteration of cell wall structural components is often detrimental to biomass production. However, the molecular mechanisms responsible for these negative effects are largely unknown. Arabidopsis (Arabidopsis thaliana) plants with altered pectin composition because of either the expression of the Aspergillus niger polygalacturonase II (AnPGII; 35S:AnPGII plants) or a mutation in the QUASIMODO2 (QUA2) gene that encodes a putative pectin methyltransferase (qua2-1 plants), display severe growth defects. Here, we show that expression of Arabidopsis PEROXIDASE71 (AtPRX71), encoding a class III peroxidase, strongly increases in 35S:AnPGII and qua2-1 plants as well as in response to treatments with the cellulose synthase inhibitor isoxaben, which also impairs cell wall integrity. Analysis of atprx71 loss-of-function mutants and plants overexpressing AtPRX71 indicates that this gene negatively influences Arabidopsis growth at different stages of development, likely limiting cell expansion. The atprx71-1 mutation partially suppresses the dwarf phenotype of qua2-1, suggesting that AtPRX71 contributes to the growth defects observed in plants undergoing cell wall damage. Furthermore, AtPRX71 seems to promote the production of reactive oxygen species in qua2-1 plants as well as plants treated with isoxaben. We propose that AtPRX71 contributes to strengthen cell walls, therefore restricting cell expansion, during normal growth and in response to cell wall damage.

The cell wall is a complex, multifunctional and dynamic structure that provides mechanical support to plant cells, and it is involved in cell adhesion, defense against pathogens, regulation of metabolic functions, and cell-to-cell communication (Keegstra, 2010). Cell walls are usually composed of polysaccharides (cellulose, hemicelluloses, and pectins), phenolic compounds (e.g. ferulic acid and lignin), and proteins (Carpita and McCann, 2000). In the apoplast, cellulose microfibrils are associated to hemicelluloses, such as xyloglucans (XGs), producing a network embedded in a matrix of pectins. The latter are mainly composed of linear chains of homogalacturonan (HG) and branched chains of rhamnogalacturonans. Pectins are abundant in the middle lamella, where they ensure cell adhesion, as well as in primary and, to a lesser degree, secondary walls (Willats et al., 2001). HG is synthesized in a highly esterified form in the Golgi apparatus (Zhang and Staehelin, 1992) and then secreted in the apoplast, where pectin methylesterases remove part of the methyl groups (Pelloux et al., 2007). Free carboxylic groups allow the formation of so-called egg box structures, in which adjacent HG chains are linked by calcium-mediated ionic bridges, making the pectin matrix more rigid (Micheli, 2001). Pectins can also form other types of interactions, such as covalent cross links with other cell wall polysaccharides, phenolic compounds, and proteins (Caffall and Mohnen, 2009; Tan et al., 2013).

The wall structure influences both the extent and the direction of cell expansion (Mirabet et al., 2011). Growth takes place perpendicularly to the direction of cellulose microfibrils, which are deposited along the perpendicular axis of the cell, providing resistance to turgor pressure and extensibility along the longitudinal axis (Crowell et al., 2010). Two major classes of proteins have been proposed to promote cell wall expansion: XG endotransglycosylases, which cleave XG chains and link together the newly generated reduced end to a new XG chain (Fry et al., 1992), and expansins, which promote primary cell walls relaxation by disrupting cellulose-hemicellulose noncovalent links (Cosgrove, 2000). During expansion, the cell wall is relaxed, whereas turgor forces induce its deformation; subsequently, expansin inhibition and formation of cross links between structural proteins (such as extensins), polysaccharides, and/or monolignols cause wall stiffening and, consequently, slow down expansion (Wolf et al., 2009).

Regulation of apoplastic levels of reactive oxygen species (ROS) is important to determine cell expansion rate and organ size (Gapper and Dolan, 2006). ROS production in the cell wall is controlled, both under physiological conditions and in response to environmental stimuli, by several classes of enzymes, most prominently plasma membrane NADPH oxidases (Torres and Dangl, 2005) and class III peroxidases (CIII Prxs; Bolwell et al., 1999; Cosio and Dunand, 2009). NADPH oxidases, commonly known as respiratory burst oxidase homologs (Rbohs), are transmembrane proteins that oxidize cytoplasmic NADPH, translocate electrons across the plasma membrane, and generate superoxide radicals in the cell wall (Torres et al., 2002; Torres and Dangl, 2005). Superoxide radicals are then rapidly converted into hydrogen peroxide (H₂O₂) either spontaneously or in a reaction catalyzed by superoxide dismutases (Bolwell et al., 1999).

CIII Prxs are heme-containing enzymes secreted in the extracellular space or the vacuole, where they perform two different enzymatic cycles, namely the peroxidative and hydroxylic cycles (Welinder et al., 2002; Passardi et al., 2004). During the peroxidative cycle, the enzyme uses H₂O₂ as an oxidant in a two-step reaction to convert different substrates, including cell wall phenolic compounds and structural proteins, into free radicals that can subsequently combine together to form covalent linkages. This activity contributes to cell wall stiffening and therefore limits growth. CIII Prxs can also cause cell wall loosening through the hydroxylic cycle, in which H₂O₂ and O₂  ⁻ are used in a Fenton-type reaction to generate hydroxyl radicals, including ^•OH, that lead to nonenzymatic cleavage of polysaccharides (Chen and Schopfer, 1999; Dunand et al., 2003; Passardi et al., 2005). CIII Prxs can, therefore, play opposite roles in cell expansion, being able to cause both wall stiffening and loosening, depending on the growth conditions. CIII Prxs can also generate O₂  ⁻, which is then dismutated into H₂O₂, through the oxidation of NAD(P)H. These enzymes can both positively and negatively modulate apoplastic ROS levels (Passardi et al., 2004).

The enzymatic characteristics of CIII Prxs allow them to participate in a wide range of physiological processes, including seed germination, plant growth, and elongation and defense against pathogens, as well as the catabolism of several extracellular molecules, including auxins (Hiraga et al., 2001). CIII Prxs are also involved in lignification through the H₂O₂-dependent generation of monolignol phenoxy radicals that spontaneously form lignin polymers (Marjamaa et al., 2009). Lignin monomers can also cross link cell wall polysaccharides, including pectins, through ferulate bridges or diferulate bonds formed by CIII Prxs in the presence of H₂O₂ (Iiyama et al., 1994). Notably, in some plant species, CIII Prxs-mediated cross links between ferulic acid and pectins arrest cell expansion (Iiyama et al., 1994). Lastly, CIII Prxs can cross link Tyr and Lys residues of extensins, contributing to the formation of a dense network within the cell wall (Schnabelrauch et al., 1996).

CIII Prxs likely appeared when plants colonized land and subsequently underwent a high rate of gene duplication, with the consequent increase of functional specialization (Passardi et al., 2005). For instance, the Arabidopsis (Arabidopsis thaliana) genome encodes 73 putative CIII Prxs, with various spatiotemporal expression profiles, suggesting that different isoforms play specific roles in growth, development, and adaptation to the environment (Tognolli et al., 2002; Welinder et al., 2002). In this article, we show that the Arabidopsis CIII Prx gene AtPRX71, which is strongly expressed upon loss of cell wall integrity (CWI), negatively affects growth and cell size and positively regulates ROS levels. In addition, when AtPRX71 is lacking, both ROS accumulation and growth defects caused by cell wall alterations are significantly reduced. We propose that accumulation of ROS-generating CIII Prxs is a mechanism to cope with loss of CWI both during normal development and in response to stress, leading to wall stiffening and therefore limiting cell expansion and growth.

RESULTS

Levels of AtPRX71 Transcripts Are Higher in Plants with Altered Cell Walls

We have previously shown that tobacco (Nicotiana tabacum) and Arabidopsis plants expressing an attenuated version of the Aspergillus niger polygalacturonase II (AnPGII; 35S:AnPGII plants) have a reduced content of deesterified HG and a significant reduction of growth that correlates with the levels of expression of the transgene (Capodicasa et al., 2004). Furthermore, 35S:AnPGII plants show constitutive activation of defense responses and accumulation of high levels of ROS in their tissues (Ferrari et al., 2008). To obtain insights into the mechanisms underlying the growth defect of 35S:AnPGII plants, whole-genome transcript analysis of rosette leaves of two independent transgenic lines, 35S:AnPGII 57 and 26, that show high levels of expression of the transgene (Lionetti et al., 2010) was performed using custom Arabidopsis 28K microarrays (GenBank Gene Expression Omnibus [GEO] Platform ID no. GPL15543). Differentially expressed transcripts were identified using a false discovery rate (FDR) < 0.05 and a module of logged fold change (FC) on base 2 (|log₂  FC|) ≥ 1 (GEO accession no. GSE66980). With this filtering criteria, the transcript levels of 16 genes increased, and those of 4 genes decreased in a statistically significant way in rosette leaves of both transgenic lines compared with the wild type (Table I). Gene Ontology functional categories of these genes were enriched in response to stress and defense against other organisms (P < 0.001). Notably, one-third of the genes significantly induced in both 35S:AnPGII lines compared with the wild type encoded proteins putatively involved in cell wall structure and/or ROS homeostasis, including EXTENSIN4 (EXT4; At1g76930), a pectin esterase (At4g02330), copper/zinc superoxide dismutase1 (CSD1; At1g08830), and a CIII Prx (At5g64120).

Genes differentially expressed in both 35S:AnPGII 57 and 26 plants compared with the wild type

At5g64120, which was among the genes whose expressions increased the most in 35S:AnPGII plants (Table I), encodes the apoplastic CIII Prx ATP15a/AtPRX71, previously shown to produce ROS in response to hypoosmolarity (Rouet et al., 2006) and recently implicated in the regulation of stem lignin composition (Shigeto et al., 2013, 2015). AtPRX71 is expressed under physiological conditions in rosette leaves and, to a lesser extent, roots and stems (Shigeto et al., 2015). Because we have previously observed high levels of ROS and apoplastic Prx activity in 35S:AnPGII plants (Ferrari et al., 2008), we hypothesized that AtPRX71 might contribute to the growth reduction observed in these plants by promoting ROS production. This gene was, therefore, selected for further characterization.

Higher levels of AtPRX71 transcripts in rosette leaves of 35S:AnPGII 57 plants compared with the wild type were confirmed by quantitative PCR (qPCR; Fig. 1A). Moreover, AtPRX71 mRNA levels also increased in the quasimodo2-1 (qua2-1) mutant (Fig. 1A), which is impaired in a putative pectin methyltransferase and, like 35S:AnPGII plants, shows reduced levels of deesterified HG and impaired growth (Mouille et al., 2007). Moreover, AtPRX71 transcript levels increased in wild-type Arabidopsis seedlings treated with the herbicide isoxaben (IXB; Fig. 1B), which inhibits cellulose synthases and affects cellulose deposition (Scheible et al., 2001). Taken together, these data indicate that alterations in different cell wall structural components promote the expression of AtPRX71.

AtPRX71 Negatively Regulates Arabidopsis Growth

To investigate the function of AtPRX71, two independent insertion lines for this gene were isolated; these lines, named atprx71-1 and atprx71-2, carry a transfer DNA (T-DNA) insertion in the second exon and the promoter of the gene, respectively (Fig. 2, A and B). AtPRX71 transcript levels were undetectable in atprx71-1 and strongly reduced in atprx71-2 seedlings (Fig. 2C). Basal guaiacol Prx activity, which characterizes CIII Prxs, was reduced in seedlings of both mutants by about 20%, compared with the wild type (Fig. 2D). Adult atprx71-1 and atprx71-2 plants displayed enhanced rosette size (Fig. 3A) and a significant increase in both fresh (Fig. 3B) and dry (Fig. 3C) biomass. An increase in biomass was also observed in 10-d-old mutant seedlings compared with the wild type (Fig. 3D). Hypocotyls of etiolated seedlings were significantly longer in both mutants than in the wild type (Fig. 3E), whereas average length and fresh weight of floral stems of wild-type and atprx71-1 plants were not significantly different (Supplemental Fig. S1). These results indicated that AtPRX71 negatively affects Arabidopsis growth. To corroborate this conclusion, we generated transgenic plants expressing AtPRX71 under the control of the constitutive Cauliflower mosaic virus 35S promoter. Four independent 35S:AtPRX71 lines (21–24) accumulating high levels of AtPRX71 transcripts (Fig. 4A) were selected for further analysis. When grown in soil, transgenic plants had smaller, more compact rosettes compared with the wild type (Fig. 4B). Lines 22 and 24, which showed higher expression of the transgene (Fig. 4A), exhibited a marked reduction of rosette size (Fig. 4B) and a significant reduction of rosette fresh weight (Fig. 4C). These lines also accumulated very high levels of guaiacol Prx activity in their leaves (Fig. 4D) compared with untransformed plants. Taken together, these data indicate that high levels of AtPRX71 expression have a negative impact on plant growth. It has been proposed that CIII Prxs can restrict cell expansion by the formation of cell wall cross links (Passardi et al., 2004, 2005). We therefore hypothesized that the effects of AtPRX71 on Arabidopsis growth may depend on its ability to influence cell size. To verify this hypothesis, the area of the epidermal cells of rosette leaves was measured in wild-type, atprx71-1, atprx71-2, and 35S:AtPRX71 plants. Average cell area in both atprx71 mutants increased by approximately 30% with respect to the wild type, whereas 35S:AtPRX71 plants showed a reduction of cell size of 20% to 30% (Fig. 5, A–F). These results, therefore, suggest that AtPRX71 negatively regulates Arabidopsis growth, because its activity limits cell expansion.

To determine if the elevated levels of expression of AtPRX71 contribute to the dwarf phenotype observed in plants with impaired CWI, we crossed atprx71-1 and 35S:AnPGII plants; however, expression of the transgene progressively declined in the subsequent generations, likely as a consequence of gene silencing, and homozygous F3 double-mutant plants did not show detectable PG activity (data not shown). For this reason, we crossed atprx71-1 with qua2-1 and analyzed the growth of homozygous double-mutant plants. Rosettes of soil-grown atprx71-1 qua2-1 plants were bigger (Fig. 6A), and rosette fresh weight was almost 4 times greater (Fig. 6B) than in single qua2-1 mutants. Hypocotyls of etiolated seedlings were also significantly longer in the double mutant compared with qua2-1 seedlings (Fig. 6C). Total guaiacol peroxidase activity was higher in qua2-1 plants than in the wild type at both seedling and adult stages, whereas activity in the qua2-1 atprx71-1 double mutant was similar to that of the wild type, although not as low as in the atprx71 mutants (Fig. 7). These data indicate that high levels of AtPRX71 expression contribute to the dwarf phenotype of qua2-1 plants, likely as a consequence of increased CIII Prx activity.

We also investigated whether AtPRX71 contributes to the growth defects caused by IXB treatment. Because this inhibitor strongly impairs Arabidopsis primary root elongation (Caño-Delgado et al., 2003; Tsang et al., 2011), we measured root length of wild-type, atprx71-1, and atprx71-2 seedlings grown for 3 d in the presence of 2.5 and 10 nm  IXB. In the absence of IXB, root length was comparable in all three genotypes (Fig. 8), indicating that AtPRX71 does not play a major role in regulating the growth of this organ. However, root elongation of atprx71-1 and atprx71-2 seedlings was less inhibited by IXB compared with the wild type (Fig. 8), suggesting that increased expression of AtPRX71 triggered by the disruption of cellulose deposition contributes to restrict root growth. Transcript levels of two defense-related genes, PHYTOALEXIN DEFICIENT3 (PAD3/At3g26830), encoding an enzyme catalyzing the biosynthesis of camalexin (Zhou et al., 1999), and At1g26380 (RetOx), encoding a protein with homology to reticuline oxidases (Denoux et al., 2008), were also analyzed in wild-type, atprx71-1, and atprx71-2 seedlings to determine whether AtPRX71 is required also for IXB-induced gene expression. However, transcripts of both genes increased in response to IXB to a similar extent in wild-type and mutant plants (Supplemental Fig. S2). Therefore, partial resistance of atprx71-1 and atprx71-2 seedlings to IXB is likely not caused by an altered uptake or perception of the inhibitor. Taken together, these results lead to the conclusion that up-regulation of AtPRX71 expression contributes to the reduced growth observed in plants undergoing loss of CWI.

AtPRX71 Promotes the Accumulation of ROS in Response to Cell Wall Alterations

Because CIII Prxs can inhibit cell expansion by promoting the accumulation of H₂O₂ in the apoplast (Lu et al., 2014), we investigated whether high levels of AtPRX71 expression are associated with increased ROS accumulation. Staining of leaves of 35S:AnPGII plants with 3′,3′-diaminobenzidine (DAB) results in a strong brown coloration of the whole lamina, indicative of high levels of H₂O₂ and CIII Prxs (Ferrari et al., 2008). Here, we show that an intense DAB staining can also be observed in leaves of qua2-1 plants (Fig. 9A), indicating that accumulation of high level of H₂O₂ is a common feature of plants with altered pectin. Notably, staining of rosette leaves was strongly reduced in leaves of the atprx71-1 qua2-1 double mutant compared with qua2-1 plants (Fig. 9A). This observation suggests that elevated levels of expression of AtPRX71 are at least partially responsible for the accumulation of ROS caused by altered pectin composition. Consistently, leaves of 35S:AtPRX71 plants showed a strong DAB staining (Fig. 9B), supporting the conclusion that high levels of expression of AtPRX71 promote the accumulation of ROS.

It has been reported that IXB induces the accumulation of H₂O₂ in Arabidopsis seedlings and that this accumulation is dependent on the NADPH oxidase AtrbohD (Denness et al., 2011). To determine whether AtPRX71 also contributes to this IXB-induced oxidative burst, wild-type and atprx7-1 seedlings were treated with IXB using the atrbohD mutant as a negative control. H₂O₂ started to accumulate in the wild type 3 to 4 h after treatment and steadily increased at least for the subsequent 14 to 15 h, whereas as expected, its accumulation was completely abolished in atrbohD seedlings (Fig. 9C). H₂O₂ production in atprx71-1 and wild-type seedlings was comparable during the first 10 to 12 h of treatment, but then it increased much more slowly in the mutant, and after 18 h of treatment it was about one-half of that observed in the wild type (Fig. 9C). This observation leads to the conclusion that AtPRX71 is not necessary for the initial onset of the IXB-induced oxidative burst, but it is required to ensure a sustained production of high levels of H₂O₂ in the apoplast. Taken together, these data indicate that AtPRX71 contributes to the accumulation of ROS in plants with altered cell walls.

Production of ROS mediated by AtPRX71 may affect not only growth but also resistance to biotic stresses. Indeed, it was previously reported that Arabidopsis plants overexpressing AtPRX71 show increased resistance to the fungus Botrytis cinerea (Chassot et al., 2007), suggesting that this CIII Prx can protect against pathogen infections. However, susceptibility of both atprx71-1 and atprx71-2 mutants to B. cinerea was comparable with that of the wild type (Supplemental Fig. S3), indicating that lack of AtPRX71 alone is not sufficient to impair resistance to this fungus.

DISCUSSION

The plant cell wall is constantly subjected to modification and reorganization, both under physiological conditions and in response to abiotic and biotic stresses (Cheung and Wu, 2011). These changes allow cells to adapt their shape and size during development and in response to environmental stimuli. However, changes in cell wall composition can have detrimental effects, and plants, therefore, must constantly adjust cell walls to maintain their mechanical properties. Increasing evidence indicates that plants possess one or more mechanisms to perceive changes in the wall that may undermine its integrity and activate proper responses, including new structural modifications aimed at maintaining CWI (Hamann, 2012). CIII Prxs are likely among the effectors of this CWI maintenance system, contributing to strengthen the cell wall and, as a consequence, limiting cell expansion and plant growth. Indeed, CIII Prxs play important roles in the regulation of cell wall mechanical properties and cell expansion (Passardi et al., 2004, 2005). Here, we have shown that expression of an Arabidopsis gene encoding a CIII Prxs, namely AtPRX71, is elevated in plants with altered pectin composition (35S:AnPGII and qua2-1 plants) or impaired in cellulose deposition (plants treated with IXB) and that lack of AtPRX71 partially restores growth defects observed in these plants. Moreover, AtPRX71 limits growth not only upon alterations of CWI but also under physiological conditions. Finally, AtPRX71 likely acts by promoting the accumulation of apoplastic ROS, which in turn may catalyze the formation of cross links, therefore stiffening the cell wall and restricting cell expansion.

The conclusion that AtPRX71 encodes a CIII Prx that negatively affects growth is based on the observations that reduced expression of this gene leads to both reduced levels of peroxidase activity and increased rosette size and biomass, whereas 35S:AnPGII plants show high levels of peroxidase activity and a significant reduction of biomass. Our findings are in agreement with previous reports describing other Arabidopsis CIII Prxs having negative effects on growth. For instance, overexpression of AtPRX37 causes dwarfism (Pedreira et al., 2011), and plants mutated for or overexpressing AtPRX53 exhibit longer or shorter hypocotyls, respectively (Jin et al., 2011). We also observed enhanced hypocotyl elongation in atprx71-1 and atprx71-2 etiolated seedlings; this latter result indicates that AtPRX71 regulates plant growth by restricting cell size rather than cell number, because it has been shown that elongation of etiolated hypocotyls occurs mainly by cell expansion (Gendreau et al., 1997). This conclusion is supported by the observation that, compared with the wild type, plants with reduced or increased levels of expression of AtPRX71 display increased or decreased leaf epidermal cell size, respectively. Indeed, it has been recently reported that increased peroxidase activity is responsible for the defective cell expansion caused by the kuoda1 mutant, which is impaired in a myeloblastosis oncoprotein (MYB)-like transcriptional repressor of different CIII Prx genes (Lu et al., 2014).

In addition to its role as a negative regulator of growth during normal development, AtPRX71 seems to limit growth in plants with altered pectin composition, which was initially suggested by the elevated expression of this gene and the increased CIII Prx activity detected in 35S:AnPGII plants (Ferrari et al., 2008) and qua2-1 (this work) and subsequently, confirmed by the observation that the constitutively high peroxidase activity and the dwarf phenotype of qua2-1 plants are partially reverted by the atprx71-1 mutation. Furthermore, AtPRX71 seems to contribute to the growth defects caused by an altered cellulose deposition, because roots of atprx71 seedlings are partially resistant to the inhibitory effect of IXB. Indeed, it has been previously shown that bean (Phaseolus vulgaris) cells habituated to dichlobenil, another inhibitor of cellulose synthesis, show increased guaiacol Prx activity (García-Angulo et al., 2009). It is, therefore, likely that accumulation of CIII Prxs is a conserved response of higher plants to cell wall damage.

The effects of AtPRX71 on Arabidopsis cell expansion and growth are likely mediated by its ability to promote the accumulation of apoplastic H₂O₂. Four lines of evidence support this hypothesis: (1) leaves of plants overexpressing AtPRX71 accumulate high levels of ROS, (2) leaves of plants with altered pectin composition (35S:AnPGII plants and qua2-1) also accumulate high levels of ROS, (3) the qua2-1 atprx71-1 double mutant shows reduced ROS accumulation compared with qua2-1, and (4) production of H₂O₂ in Arabidopsis seedlings treated with IXB is partially dependent on AtPRX71. ROS-mediated cross linking of wall structural components may be directly or indirectly catalyzed by AtPRX71 and, possibly, other CIII Prx isoforms to counteract cell wall damage. This mechanism may also act during normal development; indeed, ROS homeostasis controlled by CIII Prxs has been proposed to regulate leaf size in Arabidopsis (Lu et al., 2014). Notably, AtPRX71 affects only the late phase of H₂O₂ production in response to IXB, indicating that this and possibly, other CIII Prxs may not be required for the initial onset of the oxidative burst triggered by cell wall damage, which is indeed dependent on NAPDH oxidases (Denness et al., 2011). However, CIII Prx may be necessary to maintain a robust and prolonged production of ROS for longer times after the initial burst is triggered.

The exact biochemical mechanism responsible for the effects of AtPRX71 on Arabidopsis growth still needs to be elucidated. AtPRX71 has been implicated in stem lignification, although no alterations in stem lignin content but just a slight increase in the syringyl/guaiacyl lignin ratio was observed in knockout plants for this gene (Shigeto et al., 2013). Consistently, we did not detect significant differences in stem length and weight between wild-type and atprx71 plants, confirming that AtPRX71 has a negligible role in the lignification, at least in this organ. Characterization of AtPRX71 activity in vitro, however, indicates that this protein is able to oxidize 2,6-dimethoxyphenol and syringaldazine, which are model monolignol compounds (Shigeto et al., 2014), suggesting that this PRX may promote polymerization of lignin under specific conditions or in specific tissues. Moreover, AtPRX71 is also able to form protein radicals in vitro (Shigeto et al., 2014); the significantly increased expression of EXT4 observed in 35S:AnPGII plants, therefore, suggests that AtPRX71-mediated extensin cross links may be formed in response to altered CWI to strengthen the cell wall.

In addition to their role in plant growth, ROS-producing CIII Prxs have also been implicated in defense against pathogens. In Arabidopsis, AtPRX33 and AtPRX34 contribute to a significant proportion of the H₂O₂ generated in response to microbe-associated molecular patterns and are required for resistance to different pathogens and for the activation of some defense responses (Bindschedler et al., 2006; Daudi et al., 2012; O’Brien et al., 2012) and in particular, salicylic acid-mediated gene expression (Mammarella et al., 2015). ROS generated by AtPRX33 and AtPRX34 during infection can therefore participate in Arabidopsis defense not only by promoting cell wall reinforcement but also indirectly through the modulation of the immune response. Additional CIII Prx isoforms, including AtPRX71, that are able to favor the accumulation of ROS in the apoplast, may also contribute to Arabidopsis resistance against microbes. Indeed, it was previously shown that overexpression of AtPRX71 as well as two other CIII Prx genes confers strong resistance to B. cinerea infection (Chassot et al., 2007). However, AtPRX71 is dispensable for basal resistance to this pathogen, because atprx71-1 and atprx71-2 plants show wild-type susceptibility (this work). This apparent incongruence can be explained if expression of multiple CIII Prxs is induced during infection, acting redundantly to promote ROS production and resistance to microbes. If this is the case, lack of a single isoform would not significantly decrease the plant ability to limit pathogen growth; however, overexpression of any of these Prxs would be sufficient to boost accumulation of ROS, which we have observed in the case of 35S:AtPRX71 plants, therefore conferring a strong resistant phenotype.

The results presented in this work indicate that modifications of different cell wall structural components increase the expression of AtPRX71, which in turns, leads to ROS production and cell wall reinforcement. This implies that CWI perturbations may activate common responses, regardless of the specific component that is affected. For example, alterations of different structural polysaccharides would result in cell wall weakening, which may be perceived through the stretching of the plasma membrane under the effect of turgor pressure (Hamann, 2012). Mechanosensitive channels may thus be activated and trigger downstream responses, including accumulation of CIII Prxs. This model is supported by the observation that some phenotypes induced by IXB, such as ectopic deposition of lignin, can be reverted by osmotic support (Hamann et al., 2009). Moreover, hypoosmotic stress alone can lead to AtPRX71-mediated production of ROS (Rouet et al., 2006), suggesting that changes in turgor pressure can directly induce the expression of this peroxidase. Alternatively, loss of CWI may result in the release of elicitor-active cell wall fragments, which may be responsible for the induction of AtPRX71 expression. For instance, oligogalacturonides produced by partial degradation of HG trigger the activation of several defense responses in Arabidopsis (Ferrari et al., 2013; Benedetti et al., 2015), including the expression of AtPRX71 (Ferrari et al., 2007; Denoux et al., 2008). Further studies are required to discriminate between these two hypotheses, which are not, however, mutually exclusive.

Other than providing unique insights into the biological mechanisms regulating plant growth, our findings can be relevant to improve crops dedicated to the production of biofuels and other industrial products. Increasing evidence supports the idea that targeted modifications of cell wall structural components can increase the efficiency of conversion of lignocellulosic biomasses (Chen and Dixon, 2007; Kaida et al., 2009; Selig et al., 2009; Lionetti et al., 2010). Knowledge about how to manipulate cell wall composition without detrimental effects on growth and resistance to stresses is, therefore, needed. We have previously shown that 35S:AnPGII and qua2-1 plants are more efficiently degraded by cellulase (Lionetti et al., 2010; Francocci et al., 2013), indicating that pectin composition strongly affects biomass utilization. However, a major reduction in HG content severely impairs growth, strongly limiting the application of this approach. According to the results presented here, the detrimental effects of pectin modification on growth might be avoided by reducing the expression of specific CIII Prx isoforms. Notably, we found that lack of AtPRX71 increases biomass production without negative effects on resistance to pathogens, at least in the case of B. cinerea. Because CIII Prxs also negatively regulate saccharification efficiency (Kavousi et al., 2010), crops with both targeted modifications of cell wall composition and reduced levels of selected CIII Prxs may be more efficiently processed without detrimental effects or even a positive impact on biomass production.

In conclusion, our results indicate that wall stiffening and the consequent inhibition of growth mediated by CIII Prxs like AtPRX71 may be an important component of CWI maintenance (Hamann, 2012), both during physiological developmental processes (e.g. expansion of new organs) and in response to stresses (e.g. wounding or pathogen attack). These findings provide unique insights into the mechanisms of regulation of plant growth and may be used in the development of crop varieties with improved biomass production and utilization.

MATERIALS AND METHODS

Biological Material and Growth Conditions

All Arabidopsis (Arabidopsis thaliana) plants used in this work are in the Columbia-0 (Col-0) background. Wild-type Col-0 seeds were obtained from Lehle Seeds. The insertion lines atprx71-1 (SALK_123643) and atprx71-2 (SALK_121202C) were obtained from the Salk Institute Genomic Analysis Laboratory (Alonso et al., 2003). The generation of Col-0 plants expressing the Aspergillus niger  PGII gene (35S:AnPGII plants; lines 26 and 57) and the isolation and characterization of the qua2-1 mutant have been previously described (Mouille et al., 2007; Lionetti et al., 2010).

Plants were grown in soil (Einheitserde) in a growth chamber at 22°C and 70% relative humidity with a 16-h-light/8-h-dark photoperiod using fluorescent lamps (Osram). Light intensity was about 120 μmol m⁻² s⁻¹. Before sowing, seeds were always stratified in sterile water for 3 d in the dark at +4°C.

For in vitro growth, seeds were surface sterilized as previously described (Ferrari et al., 2007) and stratified as described above. For growth on solid medium, seeds were germinated on plates containing one-half-strength Murashige and Skoog medium (MS; Murashige and Skoog, 1962) basal salts supplemented with 1% (w/v) Suc unless otherwise stated and 0.7% (w/v) plant agar, pH 5.0. For analysis of gene expression after IXB treatments, sterilized seeds were distributed in 12-well plates (about 10 seeds per well) containing 1 mL of 2.2 g L⁻¹ basal MS supplemented with 0.5% (w/v) Suc, pH 5.5. After 9 d, the medium was replaced with fresh medium, and after 1 d, seedlings were treated for 24 h with filter-sterilized 0.01% (v/v) dimethyl sulfoxide or IXB (Sigma) at the indicated concentrations.

Gene Expression Analysis

Leaves or seedlings were frozen in liquid nitrogen and homogenized with an MM301 Ball Mill (Retsch) for about 2 min at 30 Hz. Total RNA was extracted with Isol-RNA Lysis Reagent (5′-Prime) according to the manufacturer’s instructions.

Full-genome transcriptome analysis was performed on custom Arabidopsis 28K v2.0 Microarrays (GenBank GEO Platform ID no. GPL15543) synthesized using a CombiMatrix B3 Synthesizer (Combimatrix) according to manufacturer’s instructions. Total RNA (1 µg) was amplified, and 6 µg of antisense RNA was labeled using the RNA AmpULSe Amplification and Labeling Kit with Cy5 for CombiMatrix Arrays (Kreatech Biotechnology) according to the manufacturer’s instructions. Labeled samples were hybridized to the microarrays according to CombiMatrix protocols. Scanning was performed on a GenePix 4000B Scanner (Molecular Devices). Data extraction was done using Microarray Imager software (Combimatrix), and quantile normalization of data was performed using Blist v0.6 software (Combimatrix). Differentially expressed transcripts were identified using Limma R package using an FDR < 0.05 and a module of logged FC on base 2 |log₂  FC| ≥ 1 (Smyth, 2004). Expression data are available from the National Center for Biotechnology Information (GEO accession no. GSE66980). Gene Ontology categories enrichment of differentially expressed genes was determined with the aid of the AgriGO Toolkit (Du et al., 2010).

For reverse transcription PCR analysis, RNA was treated with RQ1 DNase (Promega), and first-strand complementary DNA was obtained using Improm II Reverse Transcriptase (Promega). PCR was performed using Taq DNA Polymerase (RBC-Bioscience) with primers specific for the genes of interest (Supplemental Table S1) using the following conditions: 94°C for 2 min; 28 cycles as follows: 30 s at 94°C, 30 s at 58°C, and 30 s at 72°C; and 72°C for 5 min. Real-time PCR was performed using a CFX96 Real-Time System (Bio-Rad). Complementary DNA (corresponding to 50 ng of total RNA) was amplified using GoTaq qPCR Master Mix (Promega) and 0.4 mm each primer. Expression levels of each gene, relative to UBIQUITIN5 (UBQ5) were determined using a modification of the method by Pfaffl (2001)) as previously described (Ferrari et al., 2006).

Plant Growth Measurement

Rosette fresh weight was measured in 4-week-old soil-grown plants. Dry weight measurements were performed on the same material after incubation for 8 h at 60°C. Fresh weight of seedlings was determined after 10 d of growth in solid MS.

For measurements of hypocotyls in etiolated seedlings, sterilized seeds were sown on solid MS containing 1% (w/v) plant agar. Plates were incubated for 4 h under constant light at 25°C, wrapped with aluminum foil, and transferred to a growth chamber. Hypocotyl length was measured after incubation in the dark at 22°C for 5 d.

For cell area determination, the fifth leaf of 3-week-old soil-grown plants (at least four plants for genotype) was harvested, and chlorophyll was extracted in 100% boiling ethanol. Cleared leaves were stained with 0.05% (w/v) ruthenium red. Excess dye was removed by washing leaves with water. Leaves were mounted in 20% (v/v) glycerol and examined using a Nikon Eclipse E200 Microscope. Images were taken with a Nikon Digital Sight DS-Fi1c Camera, and cell area was measured using ImageJ (http://rsbweb.nih.gov/ij/index.html).

Fungal Infections

Growth of Botrytis cinerea and inoculation of Arabidopsis leaves were conducted as previously described (Ferrari et al., 2003).

Isolation and Genotyping of Mutants

Genomic DNA was extracted from 4-week-old plants using the method by Edwards et al. (1991). Genomic DNA was subjected to PCR to detect the wild-type allele of AtPRX71 using 71-1RP and 71-1LP primers (Supplemental Table S1) for atprx71-1 and 71-2RP and 71-2LP for atprx71-2. To detect the insertion of the T-DNA, the Lba1 primer (Supplemental Table S1) was used in place of the LP primer. Samples were subjected to amplification using Taq DNA Polymerase (RCB-Bioscience) under the following conditions: 2 min at 94°C; 35 cycles as follows: 30 s at 94°C, 30 s at 60°C, and 45 s at 72°C; and 7 min at 72°C. PCR products were separated by agarose gel electrophoresis and visualized by ethidium bromide staining.

Generation of double atprx71-1 qua2-1 mutants was achieved by crossing of single-mutant plants. F2 individuals were screened for the atprx71-1 mutation as described above, whereas the qua2-1 mutation was detected by high-resolution DNA melting analysis (Vossen et al., 2009). Briefly, genomic DNA was amplified by real-time PCR as described above with the QUA2FW and QUA2REV primers (Supplemental Table S1) using an annealing temperature of 59°C. Melting curves of the PCR products from 70°C to 80°C were obtained using 0.2°C increments in temperature at each fluorescence measurement step.

Generation of Plants Overexpressing AtPRX71

The AtPRX71 genomic region, starting from the predicted translation start codon and ending in correspondence of the predicted translation stop codon, was amplified using Col-0 genomic DNA as a template. PCR was performed with High-Fidelity PCR Master Mix (Roche) using the OEXPOX1FW and OEXPOX1REV primers (Supplemental Table S1). The purified PCR fragment was cloned into the pGEM T-Easy Vector (Promega), and the obtained plasmid was introduced in Escherichia coli DH5α by electroporation. The insert was excised from the plasmid using XbaI and SacI (Fermentas), gel purified, and subcloned into the binary vector pBI121 (Stratagene) in place of the beta-glucuronidase uidA gene. After ligation and electroporation into E. coli DH5α cells, the obtained plasmid (pBI121-AtPRX71), which contains the AtPRX71 gene under the control of the Cauliflower mosaic virus 35S promoter, was introduced in Agrobacterium tumefaciens GV3101 cells. Arabidopsis Col-0 plants were transformed with the obtained bacterial strain using the floral dip method (Clough and Bent, 1998). Transformants were selected on solid MS plates supplemented with 50 μg mL⁻¹ kanamycin.

Oxidative Burst Assay

For determination of the oxidative burst elicited by IXB, a luminol-based protocol (Denness et al., 2011) was used. Arabidopsis seedlings were grown in sterile 96-well plates (Costar) on Gamborg’s medium supplemented with 1% (w/v) Suc, pH 5.5, for 6 d at 23°C. Before the experiment, the medium was removed, and 100 μL of assay solution (17 mm luminol [Sigma], 1 μm horseradish PRX [Sigma], and 600 nM IXB) was added to each well. Plates were placed in a GloMax 96 Microplate Luminometer (Promega), and luminescence was measured for 18 h at 10-min intervals using an integration time of 1 s.

Histochemical Analyses

For H₂O₂ visualization, rosette leaves from 4-week-old plants were incubated for 12 h in a solution containing 1 mg mL⁻¹  DAB, pH 5.0. Chlorophyll was extracted for 10 min with boiling ethanol and 2 h with ethanol at room temperature before photography (Orozco-Cardenas and Ryan, 1999).

Measurement of CIII Prx Activity

Soluble proteins were extracted from 10-d-old seedlings and 4-week-old rosette leaves by grinding in the following extraction buffer (1 mL for 100 mg of seedlings and 50 µL for 100 mg of leaves): 20 mm HEPES, pH 7.0, 1 mm EGTA, 10 mm vitamin C, and PVP PolyclarAT (100 mg g⁻¹ fresh weight). The extract was centrifuged two times (10 min at 10,000g and 4°C) to remove insoluble material. Subsequent experiments were carried out on the supernatant. The protein content was determined using the Bradford Reagent (Serva) with bovine serum albumin (Sigma-Aldrich) as a standard (Bradford, 1976). PRX activity was measured at 25°C by following the oxidation of 8 mm guaiacol (Fluka) at 470 nm in the presence of 2 mm  H₂O₂ (Carlo Erba) in a phosphate buffer (200 mm, pH 6.0).

Sequence data from this article are as follows: At5g64120 (AtPRX71), At3g62250 (UBQ5), At3g26830 (PAD3), and At1g26380 (RetOx).

Supplemental Data

The following supplemental materials are available.

• Supplemental Figure S1. Lack of AtPRX71 does not affect stem growth.

• Supplemental Figure S2. Gene expression induced by IXB is not altered in atprx71 plants.

• Supplemental Figure S3. AtPRX71 is not required for basal resistance to B. cinerea.

• Supplemental Table S1. Primers used in this work.

ACKNOWLEDGMENTS

We thank Dr. Grégory Mouille and Stéphane Verger (Institut National de la Recherche Agronomique, Centre de Recherche de Versailles-Grignon, France) for providing qua2-1 seeds and assistance in the genotyping of this mutant.

Glossary

 
• Col-0

  Columbia-0

 
• CWI

  cell wall integrity

 
• DAB

  3′,3′-diaminobenzidine

 
• FC

  fold change

 
• FDR

  false discovery rate

 
• GEO

  Gene Expression Omnibus

 
• H₂O₂

  hydrogen peroxide

 
• HG

  homogalacturona

 
• IXB

  isoxaben

 
• MS

  Murashige and Skoog medium

 
• qPCR

  quantitative PCR

 
• ROS

  reactive oxygen species

 
• T-DNA

  transfer DNA

 
• XG

  xyloglucan

LITERATURE CITED

Author notes