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Activation of the Jasmonic Acid Pathway by Depletion of the Hydroperoxide Lyase OsHPL3 Reveals Crosstalk between the HPL and AOS Branches of the Oxylipin Pathway in Rice

  • Xiaoqiang Liu ,

    Contributed equally to this work with: Xiaoqiang Liu, Feng Li

  • Feng Li ,

    Contributed equally to this work with: Xiaoqiang Liu, Feng Li

  • Jiuyou Tang,
  • Weihong Wang,
  • Fengxia Zhang,
  • Guodong Wang,
  • Jinfang Chu,
  • Cunyu Yan,
  • Taoqing Wang,
  • Chengcai Chu ,

    ccchu@genetics.ac.cn (CC); cyli@genetics.ac.cn (CL)

    Affiliation State Key Laboratory of Plant Genomics, National Centre for Plant Gene Research, Institute of Genetics and Developmental Biology, Chinese Academy of Sciences, Beijing, People's Republic of China

  • Chuanyou Li

    ccchu@genetics.ac.cn (CC); cyli@genetics.ac.cn (CL)

    Affiliation State Key Laboratory of Plant Genomics, National Centre for Plant Gene Research, Institute of Genetics and Developmental Biology, Chinese Academy of Sciences, Beijing, People's Republic of China

Abstract

The allene oxide synthase (AOS) and hydroperoxide lyase (HPL) branches of the oxylipin pathway, which underlie the production of jasmonates and aldehydes, respectively, function in plant responses to a range of stresses. Regulatory crosstalk has been proposed to exist between these two signaling branches; however, there is no direct evidence of this. Here, we identified and characterized a jasmonic acid (JA) overproduction mutant, cea62, by screening a rice T-DNA insertion mutant library for lineages that constitutively express the AOS gene. Map-based cloning was used to identify the underlying gene as hydroperoxide lyase OsHPL3. HPL3 expression and the enzyme activity of its product, (E)-2-hexenal, were depleted in the cea62 mutant, which resulted in the dramatic overproduction of JA, the activation of JA signaling, and the emergence of the lesion mimic phenotype. A time-course analysis of lesion formation and of the induction of defense responsive genes in the cea62 mutant revealed that the activation of JA biosynthesis and signaling in cea62 was regulated in a developmental manner, as was OsHPL3 activity in the wild-type plant. Microarray analysis showed that the JA-governed defense response was greatly activated in cea62 and this plant exhibited enhanced resistance to the T1 strain of the bacterial blight pathogen Xanthomonasoryzaepvoryzae (Xoo). The wounding response was attenuated in cea62 plants during the early stages of development, but partially recovered when JA levels were elevated during the later stages. In contrast, the wounding response was not altered during the different developmental stages of wild-type plants. These findings suggest that these two branches of the oxylipin pathway exhibit crosstalk with regards to biosynthesis and signaling and cooperate with each other to function in diverse stress responses.

Introduction

Plants have evolved complex signaling pathways to coordinate effective responses to biotic and abiotic challenges, and to developmental stimuli. The oxylipin pathway, which induces the synthesis of biologically active metabolites called oxylipins upon activation by various stimuli, is a lipid-based signaling network. The pathway is composed of several competing branch pathways that play pivotal roles in an array of biological functions, including reproduction, in responses to biotic and abiotic stresses, in metabolic processes and in developmental regulation. Oxylipin biosynthesis is initiated by the coordinated action of lipases and lipoxygenases, which generate highly active hydroperoxy fatty acids, including 9-/13-hydroperoxy-octadecadienoic acids (9-/13-HPODs) and 9-/13-hydroperoxy-octadecatrienoic acids (9-/13-HPOTs) [1]. These hydroperoxides are substrates for a group of enzymes present in four different branches of the pathway, namely, peroxygenase (POX), divinyl ether synthase (DES), allene oxide synthase (AOS) and hydroperoxide lyase (HPL) [1], [2]. Among these, the AOS and HPL branches, which are responsible for the production of jasmonates and aldehydes, respectively, are the best studied and are known to be involved in multiple developmental and defense pathways, especially those involved in herbivore resistance, disease resistance and general stress responses [1], [3].

A large body of genetic and molecular evidence shows that jasmonates play a central role in plant defense responses to pathogen infection and insect herbivory [3], [4]. Genetic evidence for the role of jasmonic acid (JA) in defense signaling mostly comes from research on Arabidopsis thaliana mutants impaired in JA biosynthesis or perception, which lack effective defense responses against pathogen infection [5][9]. In addition, Arabidopsis mutants with constitutive activation of the JA signaling pathway (e.g., cev1) display enhanced resistance to bacterial and fungal pathogens [10], [11]. Furthermore, jasmonates have also been shown to play important roles in defense responses in Solanum lycopersicum (tomato), Nicotiana tabacum (tobacco) and Solanum tuberosum (potato) plants through mutant or transgenic plant analysis [12][14]. In monocotyledonous plants, most of our information comes from studies of the effect of exogenous JA or methyl jasmonate (MeJA) treatments on the induction of defense genes, such as pathogenesis-related (PR) genes, including PR1b, PR2, PR5 and PR10 [15][17], and phytoalexins, such as sakuranetin and momilactone A in Oryza sativa (rice) leaves [18], [19]. Molecular, biochemical and pathological analyses of transgenic rice lines in which oxylipin biosynthesis genes (e.g., OsAOS2, OsOPR1 and OsHPL2) or transcription factor genes were overexpressed, revealed that JA plays a significant role in defense gene activation, and host resistance to the rice blast fungus and bacterial blight pathogen Xanthomonasoryzaepvoryzae (Xoo) [20][24]. However, the role of JA signaling in defense responses in rice is still not clear. Therefore, the role of JA in the rice defense response needs to be further elucidated through robust genetic and molecular analyses using rice mutants or transgenic lines with altered JA biosynthesis or signaling pathways.

Whereas much research has focused on the functions of the jasmonates generated by the AOS branch pathway, the HPL branch pathway, which has recently been implicated in plant defense processes, is not fully characterized. Several studies have suggested that crosstalk exists between these two competing branches of the oxylipin pathway. For instance, the metabolites of the HPL branch of the pathway activate defense signaling, eliciting the accumulation of phytoalexins in Gossypium hirsutum L. (cotton) [25], producing anthocyanins in Arabidopsis [26], and resulting in the accumulation of the systemin precursor in Solanum lycopersicum (tomato) [27]. C6 volatiles up-regulated the expression of some defense genes involved in phenylpropanoid and oxylipin synthesis in Arabidopsis [28] and Citrus jambhili [29]. HPL genes are induced by mechanical wounding [30], [31], and expression varies greatly with developmental stage and tissue type [32], [33]. Because the accumulation of induced transcripts is not correlated with instant responses in downstream products, posttranscriptional control mechanisms, involving substrate availability or compartmentation, are expected to be involved in the regulation of HPL expression [32], [34]. The HPL gene family can be classified into two groups, 13-HPLs and 9-/13-HPLs, based on the substrate specificities. HPL acts on 13-HPOT/HPOD to yield the C6 aldehydes, i.e., hexenals and hexanals, which have been suggested to play signaling roles in plant defense processes [26], especially those involved in herbivore resistance [35], disease resistance [36] and plant-insect communication [37]. The functional roles of the HPL branch of the pathway have also been genetically manipulated in transgenic plants in which HPL activity was silenced [38], [39]. For example, antisense-mediated HPL depletion in transgenic potato plants resulted in impaired sucking insect aphid resistance, implying that the HPL-catalyzed production of C6 aldehydes may be a key step in a built-in resistance mechanism of plants against some sucking insect pests [38]. Furthermore, OsHPL2-overexpressing transgenic rice, in which (E)-2-hexenal accumulated abundantly, exhibited enhanced resistance to bacterial blight [23]. There was a negative correlation between the products of the AOS and HPL branches of the oxylipin pathway. An overlap of GLV- and JA-regulated transcript accumulation in the transformed antisense-NaHPL (as-hpl) and antisense-NaAOS (as-aos) plants revealed that the two signaling cascades had different roles in defense responses and suggested that crosstalk exists between these two branches of the oxylipin pathway with respect to biosynthesis and signaling [39]. However, the mechanism that regulates this crosstalk remains unknown.

Here, we identified a JA overproduction mutant, cea62, in a genetic screen for lineages with constitutively active expression of an allene oxide synthase gene in a rice T-DNA insertion mutant library. We then used a map-based cloning strategy to identify the target gene as OsHPL3. The cea62 mutant constitutively expressed OsAOS and exhibited spontaneous disease-like lesions and enhanced resistance to bacterial blight compared with the wild-type plant. Furthermore, we revealed that the mutant phenotype was correlated with increased jasmonic acid (JA) accumulation, induction of JA biosynthesis genes and activation of the JA signaling pathway. The microarray data showed that a series of defense response genes was also elevated in the mutant plant. In contrast, the HPL-derived oxylipin (E)-2-hexenal was dramatically reduced in the mutant. These results demonstrate that the OsHPL3-derived oxylipin pathway also plays an important role in normal plant growth and development, and that these processes are dramatically affected when the function of OsHPL3 is abolished. Furthermore, we investigated whether crosstalk exists between the HPL and AOS oxylipin biosynthesis and signaling pathways, especially during defense responses.

Results

Characterization of the cea62 mutant

To gain insight into the molecular basis of the JA signaling pathway in rice, we identified a novel JA overproduction mutant, cea62, by monitoring the expression of the Constitutive Expression of Allene oxide synthase gene (cea) in our rice T-DNA insertion mutant population (Oryza sativa var. Nipponbare background) [40]. The expression of OsAOS2 was greatly elevated in the cea62 mutant compared to in the wild-type plant (Fig. 1A), and the mutant showed a lesion mimic (LM) phenotype in the absence of pathogen attack (Fig. 1B, C and D). Brown lesion spots appeared on leaves about 2 weeks after sowing and gradually spread over the entire leaf surface during the subsequent developmental stages. To identify the biochemical mechanisms underlying the development of hypersensitive response (HR)-like lesions in the cea62 mutant, we examined the expression of several histochemical markers in both the cea62 mutant and wild-type plants. DAB staining, which is indicative of H2O2 accumulation, was strictly correlated with lesion formation in the cea62 mutant, whereas wild-type leaves produced no H2O2 (Fig. 1E). Similarly, purple formazan precipitates formed on the cea62 mutant stained with NBT (nitro-blue tetrazolium chloride), an indicator of O2, but not on any of the wild-type leaves. Furthermore, cells at the site of lesions in the cea62 mutant stained deep blue upon trypan blue staining, which indicates irreversible membrane damage or cell death, whereas the leaves of wild-type plants did not stain with trypan blue (Fig. 1E). These data suggest that reactive oxygen species (ROS) in the mutant leaves induced the HR-like cell death and are responsible for the lesion mimic phenotype. JA production was increased hundreds of times (Fig. 1F). Furthermore, the cea62 plants have reduced stature, a decreased tiller number and a decreased seed setting ratio, which is mainly due to decreased pollen fertility compared with that of the wild-type plant (Fig. 1G–I, and Fig. S1A, B).

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Figure 1. Phenotype of the cea62 mutant.

OsAOS2 expression was strongly induced in the cea62 mutant (A). Two-month-old plants (B), tillers (C) and leaves (D) of the wild type (WT) and cea62 mutant. (E) The expression of several histochemical markers in cea62 and wild-type plants was analyzed. Leaves were stained with DAB, NBT or trypan blue at 21 or 30 days after sowing. And JA production (F) was much greater in the cea62 mutant than in the wild type. (G–I) Quantification of several agricultural traits, including tiller number (G), seed setting ratio (H), and relative pollen activity (I). Each bar is the mean ± SD of 30 replicate samples.

https://doi.org/10.1371/journal.pone.0050089.g001

Map-based cloning of CEA62 and its expression patterns

Genetic analysis revealed that cea62 was caused by a single recessive nuclear gene mutation that did not co-segregate with the T-DNA insertion (data not shown). Therefore, we used map-based cloning to isolate the underlying gene. An F2 mapping population was constructed by crossing cea62 (Japonica) and Minghui 63 (Indica). Using 1200 F2 plants, the candidate gene was narrowed down to a 37-kb region between markers S2-570 and S2-632 on chromosome 2 (Fig. 2A). There are eight predicted genes within this region (Fig. 2A and Table S1). After sequencing these genes, a single-base substitution (TAC→TAG) was identified at the 1146th position of LOC_Os02g02000 in cea62, which generates a premature stop codon (Fig. 2A and Fig. S2A). To verify that Os02g02000 is CEA62, we performed a genetic complementation test in which cea62 plants were transformed with wild-type Os02g02000, which consists of 6930 bp of genomic DNA containing the entire coding region driven by its native promoter (Data S1). The resulting complemented plants are referred to hereafter as cea62-C. The transgene complemented the cea62 phenotype (Fig. 2B), confirming that Os02g02000 is indeed CEA62 and that this single-base substitution is responsible for the phenotype of cea62 plants. CEA62 encodes a cytochrome P450 family protein, which is a hydroperoxide lyase, OsHPL3 [41]. OsHPL3 is predicted to encode a polypeptide of 488 amino acids and is classified as a 13-HPL [30], [31], as it uses 13-hydroperoxides as substrates [41]. Three HPLs are present in the rice genome, OsHPL1, OsHPL2 and OsHPL3. OsHPL3 belongs to the CYP74B subfamily and shares less sequence similarity with OsHPL1 and OsHPL2, which belong to the CYP74C subfamily (Fig. S2B). Real-time PCR analysis showed that OsHPL3 transcripts were totally abolished in the cea62 mutant and were almost at wild-type levels in the complemented cea62 transgenic plant (cea62-C) (Fig. 2C). We propose that a mechanism of non-sense mediated decay (NMD) plays a role in this abnormal mRNA clearance. The organ-specific expression pattern of OsHPL3 was further examined. OsHPL3 was expressed in leaf blades and weakly in leaf sheaths, but was not expressed in culms, panicles and roots (Fig. 2D). These data confirm that OsHPL3 is CEA62 and that depletion of OsHPL3 caused the phenotype of the cea62 mutant.

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Figure 2. Molecular identification of the cea62 mutant.

(A) Map-based cloning of cea62. The CEA62 gene (red arrow) was mapped to the short arm of chromosome 2 between markers S2-570 and S2-630 and was delimited to a 37-kb region with eight candidate genes. A single-base substitution (TAC→TGA) at the 1146th position of LOC_Os02g02000 was present in the cea62 mutant. (B) Functional complementation of the cea62 mutant. Three-month-old wild type, cea62 and complemented cea62 (cea62-C) plants are shown. (C) Expression of OsHPL3/CEA62 in the wild type (WT), cea62 mutant and cea62-C plants and (D) expression of OsHPL3/CEA62 in different tissues of the unwounded wild type, as analyzed by quantitative RT-PCR. Rice OsACT was used as an internal control. These data were obtained from three independent replicates. Each bar is the mean ± SD of three replicate samples.

https://doi.org/10.1371/journal.pone.0050089.g002

Mutation of OsHPL3 causes a reduction in C6 Aldehyde and JA accumulation in cea62 plants

OsHPL3 transcripts were almost abolished in the cea62 mutant. Consequently, we propose that the ability of OsHPL3 to metabolize the cleavage of 13-hydroperoxides is greatly impaired in cea62 plants. We detected OsHPL3 enzyme activity using 13-HPOT as a substrate in the cea62 mutant, and found that enzyme lysate of cea62 plants largely failed to degrade 13-HPOT, whereas 13-HPOT was metabolized quite well by enzyme lysate extracted from the wild-type and complemented lines (Fig. 3A). This result indicates that mutation of the OsHPL3 gene abolished OsHPL3 enzyme function in the cea62 mutant. We also used 13-HPOD as a substrate to perform the same enzyme assay. No enzyme activity was detected for the wild type, cea62 mutant and cea62-C when 13-HPOD was used as substrate (Fig. 3B).

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Figure 3. In vitro enzyme activity assays of OsHPL3 and quantification of C6-aldehydes and JA.

(A) OsHPL3 activity was monitored by the loss of absorbance of substrate at 234 nm in leaf extracts of the wild type (WT), cea62 mutant and cea62 complemented transgenic plant (cea62-C) using 13-hydroperoxylinolenic acid (13-HPOT) or (B) 13-hydroperoxylinoleic acid (13-HPOD) as substrate. Results were obtained from one experiment with three biological replicates, and similar results were obtained in three independent experiments. (C) The levels of n-hexanal and (E)-2-hexenal in the WT, cea62 and cea62-C. (D) The quantity of JA in the WT and cea62 mutant. Histograms are the average of triplicate assays and the bars indicate SD.

https://doi.org/10.1371/journal.pone.0050089.g003

We next quantified the HPL pathway metabolites, i.e., the C6 aldehydes hexanal and hexenal, in the cea62 mutant, wild type and cea62-C. The OsHPL3 mutation resulted in a significant reduction in the level of (E)-2-hexenal in the cea62 mutant compared with in wild-type and cea62-C plants (Fig. 3C). In contrast, there was no difference in the level of the product of 13-HPOD, hexanal, between the wild-type, cea62 mutant and cea62-C plants (Fig. 3C). This indicates that the mutation in OsHPL3 abolishes the ability of the encoded protein to catalyze the cleavage of 13-HPOT into (E)-2-hexenal. As the HPL pathway competes against the AOS pathway for the same substrate, 13-HPOT, it is presumed that blocking of the HPL branch would have some effect on the AOS branch pathway. However, the level of JA was 162 times greater in the cea62 mutant than in the wild-type plant (Fig. 1F). This suggests that the mechanism underlying substrate competition might not be the only cause of this significant induction of JA. These data showed that mutation of OsHPL3 not only impaired the production of its metabolites, but also induced the overproduction of JA. Furthermore, these findings suggest that crosstalk exists between HPL and AOS oxylipin biosynthesis and/or signaling pathways.

Depletion of OsHPL3 activates the JA signaling pathway in a development-dependent manner that resembles that of OsHPL3 activity in the wild type

We next examined whether the JA signaling pathway was ubiquitously activated in the cea62 mutant plant by monitoring the expression of JA signaling pathway genes. We found that the expression of a series of JA biosynthesis and signaling pathway genes, such as OsLOX, OsAOS2, OsJAZ6, OsJAZ8 and OsJAmyb, was greatly induced in cea62 plants after the LM phenotype appeared (i.e., three months after sowing). However, the expression of these JA-related genes in cea62 plants was only slightly upregulated or the same as that in wild-type and cea62-C plants before the LM phenotype appeared, two weeks after sowing (Fig. 4). Similarly, the expression of some disease-related marker genes, such as OsNPR1, OsPR1b and OsPR10, in cea62 plants exhibited the same pattern as that of JA-related genes (Fig. 4). We further monitored the expression of these genes at different developmental stages in wild-type and cea62 plants. The expression of these JA-related genes was maintained at or a little above basal levels during all of these developmental stages in the wild-type plant, whereas in the cea62 mutant plant, the expression of JA biosynthesis genes, such as OsLOX and OsAOS2, began to dramatically increase two weeks after sowing (WAS) and peaked at four weeks after sowing, before gradually declining to basal levels by fifteen weeks after sowing (Fig. 5A and B). For OsJAZ6 and OsJAZ8, there was a two-week delay in induction compared with that of JA biosynthesis genes in the cea62 plant, and the expression of these genes peaked twelve weeks after sowing (Fig. 5C and D). Furthermore, the expression of OsPR1b and OsPR10 started to increase eight weeks after sowing and peaked at twelve weeks after sowing in cea62 plants (Fig. 5E and F). These data suggest that the activation of JA biosynthesis, signaling pathway and defense response by depletion of OsHPL3 varied at different developmental stages, and was associated with the development of the lesion mimic phenotype.

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Figure 4. Expression patterns of JA-related genes in the wild type and cea62 mutant.

OsLOX and OsAOS2 are JA biosynthesis genes in rice. OsJAZ6, OsJAZ8 and OsJAmyb are JA signaling genes in rice. OsPR1b and OsPR10 are pathogen-related genes in rice. OsNPR1 is a key regulator of an SA-dependent systemic resistance gene. Rice Actin1 was used as a reference control. Leaves of the wild type (WT), the cea62 mutant at two weeks (cea62) and three months (cea62/LM) after sowing and the cea62 complemented transgenic (cea62-C) plant were used to monitor the expression of these marker genes. In all panels, the mean is based on the average of three biological repeats. Each bar is the mean ± SD of three replicate samples.

https://doi.org/10.1371/journal.pone.0050089.g004

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Figure 5. Expression patterns of OsHPL3 and JA-related maker genes in the wild type and cea62 mutant at different developmental stages.

The expression of JA biosynthesis genes, (A) OsLOX and (B) OsAOS2; JA signaling genes, (C) OsJAZ6 and (D) OsJAZ8; defense-related maker genes, (E) OsPR1b and (F) OsPR10; and (G) OsHPL3 were monitored at various time points. The enzyme activity of (H) OsHPL3 was also recorded. These data were obtained from three independent replicates. Each bar is the mean ± SD of three replicate samples.

https://doi.org/10.1371/journal.pone.0050089.g005

Previous studies showed that transgenic plants in which the HPL gene was knocked-down by RNAi or anti-sense technology did not display any developmental phenotypes [38], [39]. Furthermore, it was even concluded that HPL activity was dispensable for normal growth and development in the Arabidopsis Columbia (Col) ecotype [42]. Here, we identified a natural HPL mutant, cea62, which displayed a severe phenotype, i.e., lesions on the leaves and premature leaf senescence, in rice (Fig. 1A). This indicated that OsHPL3 plays an important role in normal rice growth and development.

To gain insight into OsHPL3 function in normal growth and development, we monitored the expression of OsHPL3 and the enzyme activity of its encoded protein at 2, 8, 12 and 15 weeks after sowing in wild-type plants. The OsHPL3 transcript level was elevated up to 8 weeks after sowing and was greatly reduced after 12 weeks in wild-type plants, but was absent in cea62 plants at all developmental stages (Fig. 5G). In contrast, OsHPL3 activity was low before 8 weeks after sowing and increased greatly by 12 weeks after sowing (Fig. 5H). This result suggests that OsHPL3 expression is regulated by developmental cues at both the transcriptional and protein levels, which may involve changes in subcellular localization and protein modifications [32]. All these data demonstrate that a reduction in OsHPL3 activated JA biosynthesis, signaling and defense responses, and that this activation varied at different developmental stages in the cea62 mutant, as did the activity of OsHPL3 in the wild type. Furthermore, these data indicate that the relationship between the HPL and AOS branches of the oxylipin pathways is much more intricate than simple substrate competition, and that crosstalk exists between the transcriptional and developmental regulators of these two branches in rice.

OsHPL3 depletion activates the expression of JA-regulated defense genes in cea62 plants

To examine gene expression in the cea62 mutant, we performed a cDNA microarray analysis of rice. We sought to identify genes that were differentially expressed in wild-type and cea62 plants and thus potentially arose from depletion of the OsHPL3 transcript and HPL activity. Using the Affymetrix Rice Genome Array, which contains a total of 51,279 transcripts, including 48,564 japonica transcripts and 1,260 indica transcripts, we compared the gene expression profiles in leaf tissues of the cea62 mutant and wild-type plant after the lesion mimic phenotype appeared two months after sowing (Fig. S3). Table S2 shows that 1686 expressed transcripts (2-fold cutoff, p-values<0.05) were detected. Of these transcripts, 1352 were up-regulated and 334 were down-regulated in the cea62 mutant compared with those in the wild-type plant (Table S2). Functional classification of the differentially expressed genes revealed that the most significant difference in the gene expression profiles was that the defense responsive genes were greatly activated. These genes included a batch of pathogenesis and disease resistance-related genes, such as PAL, GST, PRs, NPR1, and dozens of WRKY transcription factor genes, together with a series of genes involved in JA biosynthesis and signaling pathways (Table 1). We also noticed that ethylene and gibberellin response genes, such as GA20ox, GID1, ERF2, ERF3, and ACC oxidase gene, were significantly induced in the mutant (Table 1). Interestingly, some abiotic responsive genes, such as salt- and drought-induced and ABA responsive genes, were greatly induced in cea62 (Table 1). We further verified the microarray data by real-time quantitative PCR of these genes (Fig. S4). These data suggest that JA-regulated defense responses are significantly activated in the cea62 mutant.

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Table 1. Selected differentially expressed genes functionally classified in the cea62 mutant compared with the wild type by microarray analysis.

https://doi.org/10.1371/journal.pone.0050089.t001

The cea62 mutant has enhanced resistance to rice bacterial blight (Xoo) infection

To test the disease resistance of cea62 plants, we infected wild-type leaves and the leaves of cea62 plants that lacked lesion mimic spots with bacterial blight pathogen Xanthomonasoryzaepvoryzae (Xoo) T1 strain at about two months after sowing. The cea62 plants were highly resistant to the T1 strain, whereas the wild-type plants were not. Twenty days after inoculation, the average lesion length on the leaves of the cea62 mutant was 1.9±1.3 cm, whereas it was 11.6±2.3 cm on those of the wild type (Fig. 6). These data indicate that the pathogen defense response was dramatically activated in cea62 mutant plants.

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Figure 6. Disease resistance test to rice bacterial blight Xanthomonasoryzaepvoryzae (Xoo) T1 strains.

Photographs were taken at 20 days after inoculation. (A) Lesion lengths on leaves of wild-type (WT) and cea62 plants at 20 days after inoculation. (B) Data represented here were obtained in one experiment with 30 biological replicates, and similar results were obtained in three independent experiments. Asterisks indicate significant differences in the cea62 mutant compared with WT plants. (*P<0.05; **P<0.01; Student's t test). Scale bars, 1 cm.

https://doi.org/10.1371/journal.pone.0050089.g006

The reduced wounding response in cea62 plants could be recovered by high levels of JA

Previous studies suggested that the expression of HPL genes was regulated by wound-induced transcriptional activation [30], [43]. HPL-derived oxoacid traumatin was identified as a wound hormone that triggers cell division at wound sites [38]. OsHPL3 transcripts are known to be upregulated in response to wounding [41], suggesting that OsHPL3 plays an important role in wound signaling. We thus wounded the leaves of wild-type and cea62 plants both before and after the LM phenotype appeared, and monitored the expression of wounding responsive genes. OsJAmyb is induced rapidly by JA or wounding and is involved in the JA-mediated signaling pathways in rice [44]. In the wild type, OsJAmyb and OsJAZ6 transcripts were induced 27- and 272-fold, respectively, by the wounding treatment (Fig. 7). In contrast, OsJAmyb and OsJAZ6 transcripts were induced only 5- and 75-fold, respectively, following wounding of cea62 plants that did not yet exhibit the LM phenotype. This suggests that mutation of OsHPL3 affects the wounding responses of cea62 plants (Fig. 7). After the LM phenotype appeared in cea62 plants, in which the concentration of JA was elevated, OsJAmyb and OsJAZ6 transcripts were induced 5- and 360-fold by wounding treatment, respectively (Fig. 7). This suggests that the high levels of JA in wounded cea62 plants recovered the induction of OsJAZ6, but did not recover the induction of OsJAmyb. These data imply that the AOS and HPL branches of the oxylipin pathway also undergo crosstalk in response to wounding. However, the details of this interaction are not clear.

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Figure 7. The wounding response of cea62 plants.

The expression of OsJAmyb and OsJAZ6 were monitored in wound-treated wild type (WT) and cea62 plants before and after the LM phenotype appeared. The results were obtained from three independent experiments.

https://doi.org/10.1371/journal.pone.0050089.g007

Discussion

Previous studies showed that both the AOS and HPL branches of the oxylipin pathway mediate plant responses to diverse biotic and abiotic stresses [1], [2] and suggested that regulatory crosstalk may exist between these branches of the pathway with respect to biosynthesis and signaling [39]. However, this possibility has not been supported by direct evidence. Here, we identified a natural HPL-depleted mutant in which JA production was dramatically increased and JA signaling was activated. Furthermore, activation of JA biosynthesis and signaling by OsHPL3 depletion varied at different developmental stages. The activation of JA signaling in turn elevated the defense responses and enhanced resistance to Xoo in the mutant plant. These findings suggest that these two branches of the oxylipin pathway cooperate with each other to contend with various environmental stresses and greatly advance our understanding of the relationship between these two branches of the oxylipin pathway. In addition, the cea62 mutant identified here will provide valuable genetic tools to further dissect the complex interplay in oxylipin-mediated signaling networks.

We demonstrated that OsNPR1 expression was induced in a development-dependent manner, as were JA-related genes, in cea62 plants (Fig. 5). NPR1 was previously shown to function as a key regulator of salicylic acid (SA)-regulated systemic acquired resistance (SAR) in Arabidopsis, and transgenic rice plants overexpressing OsNPR1 exhibited the lesion mimic phenotype and enhanced disease resistance to the Xoo pathogen [45], [46]. To verify that SA signaling is involved in generating the cea62 phenotype, we monitored the expression of SA-related genes, such as OsEDS1 and OsPAD4 [46], in the cea62 mutant. There was no difference in the expression of these genes during different developmental stages, in either the wild type or the mutant (Fig. 8A and B). We then detected the SA and JA levels in wild-type and cea62 plants before and after the LM phenotype appeared. The SA level in cea62 plants was found to be 1.6 times higher than that in the wild type at two weeks after sowing, and 2.5 times higher at two months after sowing (Fig. 8C). SA levels were lower at two months after sowing than at two weeks after sowing, in both the wild type and cea62 mutant (Fig. 8C). In the cea62 mutant, JA levels were 15 times greater than in the wild-type plant at two weeks after sowing and 162 times greater at two months after sowing (Fig. 8D). In contrast, there was no difference in JA production between these two developmental stages in the wild-type plant (Fig. 8D). Combined with the gene expression data, including the microarray data, these findings suggest that SA signaling may be involved in the defense response to Xoo in cea62 plants, but that overproduction of JA and the activation of JA are mainly responsible for the mutant phenotype, including the enhanced pathogen disease resistance.

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Figure 8. The expression of SA-regulated genes and quantity of SA and JA in the leaves of the WT and cea62 mutant before and after the lesion mimic phenotype appeared.

The leaves of 2-week-old and 2-month-old wild-type (WT) and cea62 mutant plants were used to monitor the expression of the SA-regulated genes (A) OsEDS1 and (B) OsPAD4 and to quantify (C) SA and (D) JA levels. Each bar is the mean ± SD of three replicate samples.

https://doi.org/10.1371/journal.pone.0050089.g008

A series of studies revealed no obvious phenotypic differences between the HPL-depleted transgenic plants generated by anti-sense transformation and untransformed plants [23], [38], [39]. In Arabidopsis, it was demonstrated that HPL, which facilitated the production of C6 volatiles, was differentially expressed in the Columbia (Col) and Landsberg erecta (Ler) ecotypes due to a 10-nt depletion polymorphism in the first exon of the gene in the Col ecotype. This depletion eliminated the ability of the Col ecotype to synthesize full-length HPL protein and the resulting products [42]. It was concluded that HPL signaling in the Col ecotype was dispensable for normal growth and development and that HPL was not replaced by an alternate enzyme capable of cleaving 13-HPOD [42] in Arabidopsis. In contrast, the normal growth and development of the cea62 mutant was greatly affected by depletion of OsHPL3 and the cea62 mutant displayed a severe phenotype, including cell death and lesion formation in leaves, semi-dwarfism and partial sterility (Fig. 1). Most significantly, JA biosynthesis, JA signaling and defense responses were continuously activated at specific developmental stages in the cea62 mutant. A detailed inspection of differentially expressed gene profiles in cea62 and wild-type plants by microarray analysis revealed that intense defense and stress responses were constantly initiated, even in the absence of pathogen infection and abiotic stress. Most differentially expressed genes functioning in these responses encode reactive oxygen species (ROS)-generating enzymes, heat shock proteins, JA biosynthesis and signaling proteins, glutathione S-transferases, pathogenesis- and disease resistance-related proteins, ethylene and gibberellin biosynthesis and responsive proteins, and abiotic stress-induced proteins, such as ABA-, salt-, light- and drought-induced proteins (Table 1). This clearly demonstrates that the HPL branch of the oxylipin pathway is indispensable for normal growth and development in rice. Furthermore, crosstalk between the AOS and HPL branches either involving substrate competition or signaling regulation plays an important role in the adaptation to environmental cues during plant growth and development. This communication helps establish a division-of-labor mechanism whereby the AOS and HPL branches of the oxylipin pathway perform distinct biological roles to provide effective protection against various invaders at a reduced metabolic cost. Actually, it is metabolically expensive for cea62 plants in which the function of the OsHPL3 branch was eliminated to activate JA-governed defense responses in the absence of dangerous invaders. Interestingly, the cea62 mutant displayed the LM phenotype three weeks after sowing in the greenhouse, but only two weeks after sowing in the field (data not shown). All these data suggest that the function of the HPL branch of the oxylipin pathway is to sense and protect the plant against various minor environmental stresses, such as light, temperature, ozone and wounding, and further to activate and cooperate with the JA-governed defense signaling pathway in response to severe stress by communicating with the AOS branch of the pathway.

Gomi [23] reported that OsHPL2 is involved in white-backed planthopper-induced resistance to bacterial blight Xoo in rice. In addition, OsHPL2-overexpressing transgenic rice and (E)-2-hexenal-treated wild-type rice showed enhanced resistance to Xoo, which was proposed to be due to the negative effect of elevated levels of C6 volatiles and the upregulation of numerous defense-related genes on the growth of Xoo in rice [23]. Although the role of the JA signaling pathway in this interaction was not explored in that study, microarray analysis revealed that many JA-induced genes, such as JAMyb, LOX2, AOS and PR1b, were significantly induced by white-backed planthopper (WBPH) infestation [23]. The JA signaling pathway may cooperate with the HPL branch of the pathway to enhance resistance to Xoo. A recent report states that OsHPL3 functions in defense responses against different invaders [47]. The hpl3-1 mutant was susceptible to the rice brown planthopper, but had enhanced resistance to the rice striped stem borer compared with the wild type [47]. Furthermore, hpl3-1 plants showed increased resistance to bacterial blight Xoo [47]. The altered defense responses of hpl3-1 plants to different invaders were largely ascribed to the elevated JA and SA levels or changed volatile niches [48]. Actually, the SA level was constitutively elevated in the cea62 mutant, but the level of JA only increased at specific developmental stages, even in absence of an invader. Our microarray data showed that over a dozen P450 genes were differentially expressed in cea62 plants, which provides clues as to the identity of the changed volatile niche for hpl3-1 (Table 1). These data all suggest that crosstalk exists between the HPL and AOS branches of the oxylipin pathway in the plant defense response.

We have demonstrated that depletion of OsHPL3 greatly activates the JA-governed defense response in a development-dependent manner. This finding provides insight into the function of crosstalk between the HPL branch and AOS branch of the oxylipin pathway and suggests a novel strategy for manipulating rice disease resistance by modifying the communication between these two branches of the oxylipin pathway.

Materials and Methods

Plant materials and growth conditions

The rice (Oryza sativa L.) cea62 mutant is in the Nipponbare (ssp japonica) background. Rice plants were cultivated in the experimental field of the Institute of Genetics and Developmental Biology (IGDB) in Beijing. An F2 mapping population was constructed by crossing cea62 (Japonica) with Minghui 63 (Indica). Rice plants used for the treatment were grown from seed under glasshouse conditions [25°C, 60–80% relative humidity] to the five-leaf stage.

Histochemistry

Because the leaves of the cea62 mutant exhibit the lesion-mimic phenotype three weeks after sowing, leaf samples were harvested for histochemical analysis after lesions appeared (21 days and 30 days after sowing). ROS accumulation was detected as described previously [48], with some modifications. For DAB staining, which was used to detect H2O2, leaf samples were vacuum-infiltrated (three cycles of 5 min each) in 0.1% 3,3′-diaminobenzidine (DAB) containing 10 mM MES (pH 6.5), and the leaves were placed in the dark for 18 h at 28°C and cleared in boiling ethanol (95%) for 10 min. The cleared leaves were examined and photographed in 70% glycerol. Superoxide (O2) accumulation was detected by staining with 0.5% nitro blue tetrazolium (NBT). The leaves were vacuum-infiltrated (three cycles of 5 min each) in 0.5% NBT in 10 mM potassium phosphate buffer (pH 7.8) for 16 h in the dark. Reactions were stopped by transfer to 90% ethanol at 70°C until the chlorophyll was completely removed, and the cleared leaves were examined and photographed in 70% glycerol. To detect dead cells, trypan blue staining was performed on fresh leaves, as described previously [48]. Briefly, samples were immersed in lactic acid-phenol-trypan blue solution (LPTB; 2.5% trypan blue, 25% (w/v) lactic acid, 23% water-saturated phenol and 25% glycerol in H2O) at 60°C, and vacuum infiltrated (three cycles of 5 min each). Leaf samples in LPTB were boiled in water for 2 min and then cooled to room temperature. Then, samples were destained for 3 days by replacing the LPTB solution with a chloral hydrate solution (25 g in 10 ml of H2O), and then equilibrated with 70% glycerol and mounted for microscopy.

Map-based cloning of CEA62

For map-based cloning of CEA62, an F2 mapping population was constructed by crossing cea62 with the Indica cultivar Minghui 63 (MH63). The cea62 locus was first mapped between markers S2-290 and S2-827 of chromosome 2 using 368 F2 mutant plants. Another three molecular markers were developed and the underlying gene was further narrowed down to a 37-kb region using markers S2-570 and S2-632 and 1200 F2 plants. Nine predicted ORFs exist within this 37-kb interval: Os02g01960, Os02g01970, Os02g01980, Os02g01990, Os02g02000, Os02g02010, Os02g02020, Os02g02030, and Os02g02040 (Table S1). Sequencing analysis revealed that Os02g02000 contained a single base substitution.

Complementation test of the cea62 mutant

For complementation of cea62, the 6930-bp genomic DNA fragment containing CEA62 (OsHPL3) driven by its native promoter was obtained by digestion of BAC AP004752 with EcoRI and SpeI and subsequently ligated into binary vector pCambia 1300 (Data S1). The plasmid was introduced into Agrobacterium tumefaciens AGL-1 by freeze-thaw transformation. Then, the mutant cea62 callus was transformed by an Agrobacterium-mediated method as described previously [22].

Quantitative RT-PCR analysis

Total RNAs were extracted from the leaves of rice plants using a TRIzol Kit according to the user's manual (Invitrogen). Three micrograms of total RNAs was treated with DNase I and used for cDNA synthesis with M-MLV Reverse Transcriptase (Promega). Real-time PCR experiments were performed using gene-specific primers (Table S3) and LightCycler® 480 SYBR Green I Master with the LightCycler® 480 Real-Time PCR System (Roche). Rice Actin1 was used as an internal control.

Enzyme assays

The hydroperoxide-metabolizing activity of cea62 and the wild-type plant was detected by monitoring the absorbance decrease at 234 nm on The Synergy™ Mx spectrophotometer (BioTek Instruments). Enzyme assays were performed at room temperature in 1 mL of 50 mM sodium phosphate (pH 7.0) with 20 µl of crude extracts of wild-type, cea62 or cea62-C plants. Crude extracts were obtained by homogenizing the plant leaves in enzyme buffer containing 1% Triton 20 (1 g leaf tissue per 10 ml buffer), and then spinning at 14000 g for 30 minutes. Reactions were initiated by adding 15 µl of 4 mM hydroperoxide substrate solution (13-HPOT or 13-HPOD; Cayman Chemical) to the reaction system. Two control reactions were performed simultaneously, one a blank control in which the plant crude extract was omitted, and the other a sample control that lacked substrate. These experiments were performed in triplicate for each enzyme activity experiment.

Oligo DNA microarray analysis

The Affymetrix Rice Genome Array containing 51,279 transcripts, including 48,564 japonica transcripts and 1,260 indica transcripts, was used for the microarray analysis to monitor the differential expression between the wild type and cea62 mutant. Total RNAs were extracted two months after sowing from the leaf blades of the cea62 mutant that displayed the LM phenotype and from those of wild-type plants. Three replicates were performed for both the mutant and the wild type. All microarray procedures and data analyses were performed according to the manufacturer's instructions. Analysis was performed using an ANOVA-false discovery rate (ANOVA-FDR) p-value of <0.05. Spots with changes in expression were extracted based on the criterion of a twofold increase or decrease in expression. Functional classification of the differentially expressed genes was carried out using the tools for GO categories (http://plexdb.org and https://www.affymetrix.com) and revised manually.

Quantification of JA, SA and C6-aldehydes

Leaf tissues (200 mg fresh weight) from wild-type and cea62 plants were harvested and immediately frozen in liquid nitrogen. JA and SA was extracted and quantified by GC-MS as described previously [49]. C6-aldehyde volatiles in the leaf blades of rice were measured according to the method of Chehab et al. [32]. The aldehydes were quantified after careful preparation of calibration curves with n-hexanal and (E)-2-hexenal as standards.

Bacterial inoculation

To evaluate bacterial blight disease resistance, plants were inoculated with Xantho-monasoryzaepvoryzae strain T1 at the seedling stage by the leaf-clipping method [50]. Disease was scored by measuring the lesion length at 3 weeks after inoculation. Thirty leaves, obtained from 30 plants (one leaf per plant), were inoculated, measured and subjected to statistical analysis. Three independent replicates were performed.

Supporting Information

Data S1.

The Genomic DNA sequence used to complement the cea62 mutant. The genomic DNA sequence containing the OsHPL3 gene derived by its native promoter used for the complementary test was got from BAC AP004752 digested by EcoRI and SpeI.

https://doi.org/10.1371/journal.pone.0050089.s001

(DOCX)

Figure S1.

Fertility of the cea62 mutant. Pollen fertility of the wild type (A) and cea62 (B) was estimated by I2-KI solution staining. Fertile pollen stain blue. Scale bars, 50 µm. Seeds of the wild type (C) and cea62 mutant (D) plant. Scale bars, 1 cm.

https://doi.org/10.1371/journal.pone.0050089.s002

(TIF)

Figure S2.

Sequence of OsHPL3 and phylogenetic analysis of AOS and HPL proteins from Arabidopsis and rice. (A) The deduced amino acid sequences of OsHPL3. The star indicates the position of the mutated base in cea62, which forms a stop code. (B) Phylogenetic tree of reported HPL and AOS proteins in Arabidopsis and rice based on their full-length deduced amino acid sequences. Plant species and accession numbers are: AtHPL, AAC69871; AtAOS, CAA63266; OsHPL1, AK105964; OsHPL2, AK107161; OsHPL3, AY340220; OsAOS1, BAD08330; and OsAOS2, AAL17675.

https://doi.org/10.1371/journal.pone.0050089.s003

(TIF)

Figure S3.

Heat map of the microarray analysis of the cea62 plant. P-value<0.05; fold change>2.

https://doi.org/10.1371/journal.pone.0050089.s004

(TIF)

Figure S4.

Verification of the differentially expressed genes identified by microarray analysis using qPCR. A and B, JA-related genes. C, senescence-related genes. D and E, pathogenesis- and disease resistance-related genes. F, abiotic stress-related genes. G, GA-related genes. I, HSP genes. The same set of RNAs used for the microarray analysis was used to verify these genes by qPCR. The gene ID numbers and primers used to amplify these genes are provided in Table S3.

https://doi.org/10.1371/journal.pone.0050089.s005

(TIF)

Table S1.

The candidate genes between S2-570 and S2-632 in BAC AP004752. The gene locus, the start and end sites of the coding sequence and genes description for these candidate genes from gramene (http://www.gramene.org/) were listed.

https://doi.org/10.1371/journal.pone.0050089.s006

(DOCX)

Table S2.

The differentially expressed genes in the cea62 mutant identified by microarray analysis. Gene expression profiles in leaf tissues of the cea62 mutant and wild-type plant after the lesion mimic phenotype appeared two months after sowing were monitored using the Affymetrix Rice Genome Array, and 1686 differentially expressed transcripts (2-fold cutoff, p-values<0.05) were detected.

https://doi.org/10.1371/journal.pone.0050089.s007

(XLSX)

Table S3.

Gene ID numbers and primers used for quantitative PCR expression analysis. The genes ID, primer sequences and notes for those genes used in this research were listed.

https://doi.org/10.1371/journal.pone.0050089.s008

(DOCX)

Acknowledgments

We thank Gupo Li and Yongshan Wen for taking care of the rice plants in the experimental field.

Author Contributions

Conceived and designed the experiments: XL CC CL. Performed the experiments: XL FL JT WW FZ CY TW. Analyzed the data: XL GW JC. Wrote the paper: XL CC CL.

References

  1. 1. Howe GA, Schilmiller AL (2002) Oxylipin metabolism in response to stress. Curr Opin Plant Biol 5: 230–236.
  2. 2. Creelman RA, Mulpuri R (2002) The oxylipin pathway in Arabidopsis. Arabidopsis Book 1: e0012.
  3. 3. Farmer EE, Almeras E, Krishnamurthy V (2003) Jasmonates and related oxylipins in plant responses to pathogenesis and herbivory. Curr Opin Plant Biol 6: 372–378.
  4. 4. Blee E (2002) Impact of phyto-oxylipins in plant defense. Trends Plant Sci 7: 315–322.
  5. 5. Feys B, Benedetti CE, Penfold CN, Turner JG (1994) Arabidopsis Mutants Selected for Resistance to the Phytotoxin Coronatine Are Male Sterile, Insensitive to Methyl Jasmonate, and Resistant to a Bacterial Pathogen. Plant Cell 6: 751–759.
  6. 6. Stintzi A, Browse J (2000) The Arabidopsis male-sterile mutant, opr3, lacks the 12-oxophytodienoic acid reductase required for jasmonate synthesis. Proc Natl Acad Sci U S A 97: 10625–10630.
  7. 7. Thomma BP, Eggermont K, Penninckx IA, Mauch-Mani B, Vogelsang R, et al. (1998) Separate jasmonate-dependent and salicylate-dependent defense-response pathways in Arabidopsis are essential for resistance to distinct microbial pathogens. Proc Natl Acad Sci U S A 95: 15107–15111.
  8. 8. Vijayan P, Shockey J, Levesque CA, Cook RJ, Browse J (1998) A role for jasmonate in pathogen defense of Arabidopsis. Proc Natl Acad Sci U S A 95: 7209–7214.
  9. 9. Xie DX, Feys BF, James S, Nieto-Rostro M, Turner JG (1998) COI1: an Arabidopsis gene required for jasmonate-regulated defense and fertility. Science 280: 1091–1094.
  10. 10. Ellis C, Turner JG (2001) The Arabidopsis mutant cev1 has constitutively active jasmonate and ethylene signal pathways and enhanced resistance to pathogens. Plant Cell 13: 1025–1033.
  11. 11. Ellis C, Karafyllidis I, Wasternack C, Turner JG (2002) The Arabidopsis mutant cev1 links cell wall signaling to jasmonate and ethylene responses. Plant Cell 14: 1557–1566.
  12. 12. Howe GA, Ryan CA (1999) Suppressors of systemin signaling identify genes in the tomato wound response pathway. Genetics 153: 1411–1421.
  13. 13. Laudert D, Schaller F, Weiler EW (2000) Transgenic Nicotiana tabacum and Arabidopsis thaliana plants overexpressing allene oxide synthase. Planta 211: 163–165.
  14. 14. Gobel C, Feussner I, Hamberg M, Rosahl S (2002) Oxylipin profiling in pathogen-infected potato leaves. Biochim Biophys Acta 1584: 55–64.
  15. 15. Takeuchi K, Gyohda A, Tominaga M, Kawakatsu M, Hatakeyama A, et al. (2011) RSOsPR10 expression in response to environmental stresses is regulated antagonistically by jasmonate/ethylene and salicylic acid signaling pathways in rice roots. Plant Cell Physiol 52: 1686–1696.
  16. 16. Liu XQ, Bai XQ, Qian Q, Wang XJ, Chen MS, et al. (2005) OsWRKY03, a rice transcriptional activator that functions in defense signaling pathway upstream of OsNPR1. Cell Res 15: 593–603.
  17. 17. Kim SG, Kim ST, Wang Y, Yu S, Choi IS, et al. (2011) The RNase activity of rice probenazole-induced protein1 (PBZ1) plays a key role in cell death in plants. Mol Cells 31: 25–31.
  18. 18. Tamogami S, Rakwal R, Kodama O (1997) Phytoalexin production elicited by exogenously applied jasmonic acid in rice leaves (Oryza sativa L.) is under the control of cytokinins and ascorbic acid. FEBS Lett 412: 61–64.
  19. 19. Nojiri H, Sugimori M, Yamane H, Nishimura Y, Yamada A, et al. (1996) Involvement of Jasmonic Acid in Elicitor-Induced Phytoalexin Production in Suspension-Cultured Rice Cells. Plant Physiol 110: 387–392.
  20. 20. Mei C, Qi M, Sheng G, Yang Y (2006) Inducible overexpression of a rice allene oxide synthase gene increases the endogenous jasmonic acid level, PR gene expression, and host resistance to fungal infection. Mol Plant Microbe Interact 19: 1127–1137.
  21. 21. Deng H, Liu H, Li X, Xiao J, Wang S (2012) A CCCH-Type Zinc Finger Nucleic Acid-Binding Protein Quantitatively Confers Resistance against Rice Bacterial Blight Disease. Plant Physiol 158: 876–889.
  22. 22. Liu X, Bai X, Wang X, Chu C (2007) OsWRKY71, a rice transcription factor, is involved in rice defense response. J Plant Physiol 164: 969–979.
  23. 23. Gomi K, Satoh M, Ozawa R, Shinonaga Y, Sanada S, et al. (2010) Role of hydroperoxide lyase in white-backed planthopper (Sogatella furcifera Horvath)-induced resistance to bacterial blight in rice, Oryza sativa L. Plant J 61: 46–57.
  24. 24. Agrawal GK, Jwa NS, Shibato J, Han O, Iwahashi H, et al. (2003) Diverse environmental cues transiently regulate OsOPR1 of the “octadecanoid pathway” revealing its importance in rice defense/stress and development. Biochem Biophys Res Commun 310: 1073–1082.
  25. 25. Zeringue HJ Jr (1991) Effect of C6 to C9 alkenals on aflatoxin production in corn, cottonseed, and peanuts. Appl Environ Microbiol 57: 2433–2434.
  26. 26. Bate NJ, Rothstein SJ (1998) C6-volatiles derived from the lipoxygenase pathway induce a subset of defense-related genes. Plant J 16: 561–569.
  27. 27. Sivasankar S, Sheldrick B, Rothstein SJ (2000) Expression of allene oxide synthase determines defense gene activation in tomato. Plant Physiol 122: 1335–1342.
  28. 28. Kishimoto K, Matsui K, Ozawa R, Takabayashi J (2005) Volatile C6-aldehydes and Allo-ocimene activate defense genes and induce resistance against Botrytis cinerea in Arabidopsis thaliana. Plant Cell Physiol 46: 1093–1102.
  29. 29. Gomi K, Yamasaki Y, Yamamoto H, Akimitsu K (2003) Characterization of a hydroperoxide lyase gene and effect of C6-volatiles on expression of genes of the oxylipin metabolism in Citrus. J Plant Physiol 160: 1219–1231.
  30. 30. Bate NJ, Sivasankar S, Moxon C, Riley JM, Thompson JE, et al. (1998) Molecular characterization of an Arabidopsis gene encoding hydroperoxide lyase, a cytochrome P-450 that is wound inducible. Plant Physiol 117: 1393–1400.
  31. 31. Howe GA, Lee GI, Itoh A, Li L, DeRocher AE (2000) Cytochrome P450-dependent metabolism of oxylipins in tomato. Cloning and expression of allene oxide synthase and fatty acid hydroperoxide lyase. Plant Physiol 123: 711–724.
  32. 32. Chehab EW, Raman G, Walley JW, Perea JV, Banu G, et al. (2006) Rice HYDROPEROXIDE LYASES with unique expression patterns generate distinct aldehyde signatures in Arabidopsis. Plant Physiol 141: 121–134.
  33. 33. Zhu BQ, Xu XQ, Wu YW, Duan CQ, Pan QH (2012) Isolation and characterization of two hydroperoxide lyase genes from grape berries : HPL isogenes in Vitis vinifera grapes. Mol Biol Rep
  34. 34. Froehlich JE, Itoh A, Howe GA (2001) Tomato allene oxide synthase and fatty acid hydroperoxide lyase, two cytochrome P450s involved in oxylipin metabolism, are targeted to different membranes of chloroplast envelope. Plant Physiol 125: 306–317.
  35. 35. Baldwin IT, Kessler A, Halitschke R (2002) Volatile signaling in plant-plant-herbivore interactions: what is real? Curr Opin Plant Biol 5: 351–354.
  36. 36. Dong F, Yang Z, Baldermann S, Sato Y, Asai T, et al. (2011) Herbivore-induced volatiles from tea (Camellia sinensis) plants and their involvement in intraplant communication and changes in endogenous nonvolatile metabolites. J Agric Food Chem 59: 13131–13135.
  37. 37. Matsui K (2006) Green leaf volatiles: hydroperoxide lyase pathway of oxylipin metabolism. Curr Opin Plant Biol 9: 274–280.
  38. 38. Vancanneyt G, Sanz C, Farmaki T, Paneque M, Ortego F, et al. (2001) Hydroperoxide lyase depletion in transgenic potato plants leads to an increase in aphid performance. Proc Natl Acad Sci U S A 98: 8139–8144.
  39. 39. Halitschke R, Ziegler J, Keinanen M, Baldwin IT (2004) Silencing of hydroperoxide lyase and allene oxide synthase reveals substrate and defense signaling crosstalk in Nicotiana attenuata. Plant J 40: 35–46.
  40. 40. Ma Y, Liu L, Zhu C, Sun C, Xu B, et al. (2009) Molecular analysis of rice plants harboring a multi-functional T-DNA tagging system. J Genet Genomics 36: 267–276.
  41. 41. Chehab E, Raman G, Walley J, Perea J, Banu G, et al. (2006) Rice HYDROPEROXIDE LYASES with unique expression patterns generate distinct aldehyde signatures in Arabidopsis. Plant physiology 141: 121–134.
  42. 42. Duan H, Huang MY, Palacio K, Schuler MA (2005) Variations in CYP74B2 (hydroperoxide lyase) gene expression differentially affect hexenal signaling in the Columbia and Landsberg erecta ecotypes of Arabidopsis. Plant Physiol 139: 1529–1544.
  43. 43. Matsui K, Wilkinson J, Hiatt B, Knauf V, Kajiwara T (1999) Molecular cloning and expression of Arabidopsis fatty acid hydroperoxide lyase. Plant Cell Physiol 40: 477–481.
  44. 44. Lee MW, Qi M, Yang Y (2001) A novel jasmonic acid-inducible rice myb gene associates with fungal infection and host cell death. Mol Plant Microbe Interact 14: 527–535.
  45. 45. Bai W, Chern M, Ruan D, Canlas PE, Sze-To WH, et al. (2011) Enhanced disease resistance and hypersensitivity to BTH by introduction of an NH1/OsNPR1 paralog. Plant Biotechnol J 9: 205–215.
  46. 46. Pieterse CM, van der Does D, Zamioudis C, Leon-Reyes A, van Wees SC (2012) Hormonal Modulation of Plant Immunity. Annu Rev Cell Dev Biol May 3 (Epub ahead of print)..
  47. 47. Tong XH, Zhu XD, Mao BZ, Zeng LJ, Wang BH, et al. (2012) The rice hydroperoxide lyase OsHPL3 functions in defense responses by modulating the oxylipin pathway. The Plant Journal 71: 763–775.
  48. 48. Qiao Y, Jiang W, Lee J, Park B, Choi MS, et al. (2010) SPL28 encodes a clathrin-associated adaptor protein complex 1, medium subunit micro 1 (AP1M1) and is responsible for spotted leaf and early senescence in rice (Oryza sativa). New Phytol 185: 258–274.
  49. 49. Schweizer P, Buchala A, Silverman P, Seskar M, Raskin I, et al. (1997) Jasmonate-Inducible Genes Are Activated in Rice by Pathogen Attack without a Concomitant Increase in Endogenous Jasmonic Acid Levels. Plant Physiol 114: 79–88.
  50. 50. Kauffman HE, Reddy APK, Hsieh SPY, Merca SD (1973) An improved technique for evaluating resistance of rice varieties to Xanthomonas oryzae. Plant Dis Rep 57: 537–541.