Abstract
The xanthophyll cycle is involved in dissipating excess light energy to protect the photosynthetic apparatus in a process commonly assessed from non-photochemical quenching (NPQ) of chlorophyll fluorescence. Here, it is shown that the xanthophyll cycle is modulated by the necrotrophic pathogen Sclerotinia sclerotiorum at the early stage of infection. Incubation of Sclerotinia led to a localized increase in NPQ even at low light intensity. Further studies showed that this abnormal change in NPQ was closely correlated with a decreased pH caused by Sclerotinia-secreted oxalate, which might decrease the ATP synthase activity and lead to a deepening of thylakoid lumen acidification under continuous illumination. Furthermore, suppression (with dithiothreitol) or a defect (in the npq1-2 mutant) of violaxanthin de-epoxidase (VDE) abolished the Sclerotinia-induced NPQ increase. HPLC analysis showed that the Sclerotinia-inoculated tissue accumulated substantial quantities of zeaxanthin at the expense of violaxanthin, with a corresponding decrease in neoxanthin content. Immunoassays revealed that the decrease in these xanthophyll precursors reduced de novo abscisic acid (ABA) biosynthesis and apparently weakened tissue defense responses, including ROS induction and callose deposition, resulting in enhanced plant susceptibility to Sclerotinia. We thus propose that Sclerotinia antagonizes ABA biosynthesis to suppress host defense by manipulating the xanthophyll cycle in early pathogenesis. These findings provide a model of how photoprotective metabolites integrate into the defense responses, and expand the current knowledge of early plant-Sclerotinia interactions at infection sites.
Author Summary
In recent years, the role of the chloroplast in the defense against microbes has been intensively investigated and is of high interest to both plant-microbe interaction and photosynthesis research. The xanthophyll cycle is well known to be involved in dissipating excess light energy to protect the photosynthetic apparatus in a process commonly assessed via non-photochemical quenching (NPQ) of chlorophyll fluorescence. Recent studies show that NPQ can be positively or negatively affected by pathogen attack. However, knowledge about the regulatory processes by which pathogens affect NPQ, as well as their impact on plant defense responses, is incomplete. This work characterized the impact of infection of Arabidopsis leaves by the necrotrophic pathogen Sclerotinia sclerotiorum on the xanthophyll cycle. Our research revealed for the first time that Sclerotinia uses a novel strategy involving manipulation of the xanthophyll cycle to weaken host defense responses and increase its successful colonization of host cells. These findings contribute to understanding the plant-Sclerotinia interactions in early pathogenesis, which will provide new sights into the development of strategies to increase Sclerotinia resistance in plants for practical applications.
Introduction
Chloroplasts are not only the factory for photosynthesis, but are also involved in various types of plant-pathogen interactions [1–3]. Indeed, the process of photosynthesis is functionally linked to plant immunity by providing energy, reducing equivalents and carbon skeletons [4–9] as well as producing oxidants and oxidant-derived hormonal messengers with roles in defense responses [10–11]. Light energy absorbed by the harvesting antenna complexes is transferred to reaction centers to drive photochemistry. However, when the rate of excitation energy exceeds the capacity for light utilization, excited-state chlorophyll can be de-excited by thermal dissipation in a process that is commonly assessed as non-photochemical quenching (NPQ) of chlorophyll fluorescence [12–15]. Mechanisms involved in thermal energy dissipation include the xanthophylls zeaxanthin and lutein, the photosystem II subunit S (PsbS) protein, as well as energetic couplings between the core antenna complexes and LHCII [16–23]. The most rapid component of NPQ is called qE, which is activated by a decrease in thylakoid lumen pH [13,15,24–25]. In the xanthophyll cycle, low pH activates violaxanthin de-epoxidase (VDE) that converts violaxanthin into zeaxanthin via the intermediate antheraxanthin. Conversely, under low light and relatively alkaline conditions, zeaxanthin epoxidase (ZEP) catalyzes conversion of zeaxanthin via antheraxanthin into violaxanthin, thus forming an integrated cycle [26]. While there is a school of thought that addressed the zeaxanthin and PsbS-dependent qE as separate mechanisms, the elegant works by Demmig-Adams & Adams group have proposed that these are two parts of the same process, where the xanthophyll cycle generates zeaxanthin, and PsbS triggers the actual engagement of zeaxanthin in thermal dissipation [12, 27].
At present, although the xanthophyll cycle is well known to be involved in photoprotection, it has not been as deeply characterized in plant disease responses. Several recent studies, however, have shown that there is a correlation between NPQ changes and resistance to pathogens [28–32]. The deletion of PsbS in the npq4-1 mutant was shown to alter jasmonate metabolism and render plant less attractive for herbivores [28–29]. Moreover, NPQ formation is negatively correlated with reactive oxygen species (ROS) production under excess light [11,15,33], and weakening NPQ may promote 1O2 generation in PSII [26,33]. In particular, in the PsbS/vde1 double mutant, treatment with flg22 enhances ROS production and early defense marker gene expression [30]. In addition, the intensity of NPQ was also positively or negatively affected by various pathogen attacks, increasing around the infected regions but decreasing in its core [34–35]. This variability in NPQ might depend on the degree of tissue damage [35]. However, knowledge about the regulatory processes of pathogens on NPQ as well as their impact on plant defense responses is incomplete.
The xanthophyll precursor pool plays an important role in the biosynthesis of the phytohormone abscisic acid (ABA) [36–38]. De novo synthesis of ABA requires ZEP-catalyzed epoxidation of zeaxanthin to violaxanthin. Subsequently, the violaxanthin-derivatives neoxanthin and xanthoxin are converted into ABA through a series of isomerization and dehydrogenation reactions [39]. In the ABA-deficient mutant aba1 (an allele of npq2), ZEP is not functional, causes accumulation of zeaxanthinin parallel with decreases in the epoxy-xanthophylls antheraxanthin, violaxanthin and neoxanthin [40–41]. In the xanthophyll cycle, VDE requires ascorbate as a reductant to convert violaxanthin to zeaxanthin [42]. As a result, reduced levels of ascorbate in the Arabidopsis vtc1 (vitamin C1) mutant stimulate ABA production [43]. In contrast, enhanced VDE activity can reduce ascorbate levels and antagonize ABA synthesis [43]. Thus, the regulation of the xanthophyll cycle allows ABA levels to be modified, which could be a subtle mechanism exploited by pathogens to lower plant resistance.
NPQ is regulated on a fast timescale by changes in thylakoid lumen pH [15,19,44]. Disruption of the pH gradient (ΔpH) across the thylakoid membrane with the ionophore nigericin can abolish NPQ formation [45]. Conversely, NPQ can be induced in isolated thylakoids by lowering ambient pH [46,47]. In the pathogenesis of pathogenic fungi, local pH can be dynamically altered by the pathogen as host colonization advances [48]. In fact, pH value is one of the major features affecting maximal activity of pathogenicity factors, such as the arsenal of cell wall degradative enzymes that display acidic pH-specific expression in the necrotrophic pathogen Sclerotinia sclerotiorum [49,50]. Sclerotinia decreases host pH by secreting millimolar quantities of oxalate [51,52]. Oxalate exhibits versatile functions in plant infection and fungal development [53]; it triggers plant programmed cell death [54–56], suppresses plant oxidative burst and callose deposition [57–59], and inhibits ABA-induced stomatal closure [60]. Functional genetic studies have provided evidence for the relevance of ABA in plant defense against Sclerotinia [61–63]. However, it is still unknown whether the ambient pH changes would affect the xanthophyll cycle and subsequent ABA biosynthesis in the pathogenesis of Sclerotinia.
Here, we investigated the interplay of the xanthophyll cycle and plant resistance to the necrotrophic pathogen Sclerotinia. The results show that Sclerotinia caused a dysfunction of the xanthophyll cycle during initial stages of infection, with leaves displaying an abnormal increase in NPQ in a zeaxanthin-related manner even under low light conditions. Further studies revealed that decreases in the precursor violaxanthin were associated with limited ABA biosynthesis, which, in turn, apparently weakened tissue defense responses and eased Sclerotinia colonization of the host plant. These findings present a mechanism of how photoprotective metabolites integrate into the defense work and contribute to understanding the early plant-Sclerotinia interactions at the infection site.
Results
Sclerotinia infection leads to a localized increase in NPQ
When analyzing the timing and spread of Sclerotinia in its host plant with chlorophyll fluorescence imaging, we identified anomalies of NPQ in plant tissue during early infection. Fig 1A shows images of two conventional fluorescence parameters, Fv/Fm (maximum photochemical efficiency of PSII) and NPQ, in randomly selected Arabidopsis leaves. Sclerotinia infection induced a gradual decrease in Fv/Fm, which indirectly reflected the degree of tissue damage [64]. Interestingly, a localized increase in NPQ was observed already 1 h after infection. As inoculation time prolonged, NPQ decreased in the core of the necrotic lesions but increased around the necrosis. Because the infected areas did not behave homogeneously, possibly due to contact spot variances on the uneven foliage, the entire inoculated region and the leading edge were selected for statistical analysis, respectively (Fig 1B and 1C). Although the mean values of NPQ decreased significantly in severely damaged tissue (as shown at 9 h), NPQ remained at high levels from 1 to 3 h after infection (Fig 1D). The increase in NPQ was most pronounced at the leading edge (Fig 1E).
Next, changes in NPQ within the context of the penetration of the host by Sclerotinia were assessed. A water-soaked appearance began to emerge at 1 h but exhibited severely at 12 h after infection (Fig 1F). The earlier slight damage might be caused by oxalate in the PDA plug. At early stage, a number of scattered mycelial cells on the leaf surface were observed under scanning electron microscope (Fig 1G). Further results revealed that the infection cushions began forming at 8 h and hyphae were interweaved in the necrotic tissue at later stage (Figs 1G and S1). These features suggest that the Sclerotinia-induced NPQ increase is an early event that occurs prior to infection cushions formation. A model is proposed to depict how NPQ is related to the infection process (Fig 1H): During the early stage, upper-side cell damage causes a slight decrease in Fv/Fm but greatly enhances NPQ throughout the entire region. As inoculated tissue moves toward necrosis, it exhibits increased NPQ in the leading edge, whereas both Fv/Fm and NPQ are reduced in the necrotic center. This model could help explain why Sclerotinia-induced increased NPQ varies dependent on region and infection stage.
The dynamics of NPQ in Sclerotinia-infected leaves
We next analyzed the kinetic characteristics of NPQ in the Sclerotinia-infected leading edge area. First, different intensities of actinic light (levels of photosynthetically active radiation = PAR ranging from 0 to 1465 μmol photons m-2 s-1) were used to investigate dynamic changes in NPQ. As light intensity increased, a ring of enhanced NPQ was detectable surrounding the inoculated zone, and then expanded to the entire infected area (Fig 2A and S1 Movie). However, at light intensities exceeding 1175 μmol photons m-2 s-1, NPQ increased more in un-inoculated regions (Fig 2A and 2D). To analyze formation and relaxation of NPQ under excess light, a light intensity of 725 μmol photons m-2 s-1 was selected. In the Sclerotinia-infected zone, NPQ formed quickly in the first 60 seconds. In contrast, longer illumination led to greater NPQ generation in the un-inoculated control regions and with increased maximum amplitude (Fig 2B, 2E and S2 Movie). Interestingly, when the light switched off, NPQ relaxed more slowly in the infected area (Fig 2E).
Because NPQ has a dedicated function in protecting the photosynthetic apparatus against photodamage under excess light, we wanted to ascertain the impact of Sclerotinia infection on NPQ changes at the low light intensity of 133 μmol photons m-2 s-1, which was close to the natural radiation in our greenhouse. Surprisingly, even at this low light intensity, Sclerotinia infection still rapidly induced NPQ formation (Fig 2C, 2F and S3 Movie). More importantly, the maximal amplitude was approximately 2-fold of that found in un-inoculated regions (Fig 2F). Additionally, differences of NPQ relaxation kinetic between Sclerotinia-infected leaves and the control were still observed (Fig 2F). These results indicate that NPQ, usually seen under excess light conditions, was triggered by Sclerotinia invasion even at low light during early pathogenesis. To explore these effects induced by Sclerotinia under close to natural growth conditions, the low PAR of 133 μmol photons m-2 s-1 was used in the following experiments unless otherwise mentioned.
The increase of NPQ in Sclerotinia-infected area is attributed to the decreased ambient pH
Oxalate is an essential pathogenicity factor for Sclerotinia [52,57]. Inoculation with Sclerotinia induced calcium oxalate crystal accumulation in the infection sites (Fig 3A). It is controversial whether or not the dibasic acid oxalate aids in fungal invasion due to direct acidity effects. To explore whether the increased NPQ in Sclerotinia-infected zone was related to positional pH changes, two pH-sensitive fluorescent dyes, lysosensor green DND-189 and acridine orange, were used. The infected plant tissue exhibited a higher level of DND-189 fluorescence upon invasion with wild-type Sclerotinia compared to the oxalate-deficient A2 mutant (Fig 3B). Acridine orange has an emission maximum of 655 nm (red) in an acidic environment and of 530 nm (green) in a neutral environment [65]. Tissue acidification was determined by measuring the ratio of red-to-green emissions. Results obtained via confocal microscopy show that wild-type Sclerotinia infection induced a higher level of fluorescence emissions of acridine orange in the red channels (615 to 660 nm) compared to the A2 mutant. At the periphery of wild-type Sclerotinia-infected sites, the ratio of red-to-green emissions greatly increased (Fig 3C), indicating a decrease in ambient pH. We then evaluated whether loss of oxalate would affect the Sclerotinia-induced NPQ increase. One leaf was co-infected with wild-type Sclerotinia (Circle 1) and the oxalate-deficient A2 mutant (Circle 2). Chlorophyll fluorescence imaging revealed that the A2 mutant does not significantly stimulate NPQ as done by wild-type Sclerotinia (Fig 3D). The kinetics of NPQ formation and relaxation are similar in A2-inoculated leaves and controls (Fig 3E). These results suggest that acidification of the plant tissue by Sclerotinia-secreted oxalate might account for the abnormal increase in NPQ.
To further investigate the impact of ambient pH changes on NPQ kinetics, leaves were infiltrated with KOX (potassium oxalate) buffered to different pH values. A rapid increase in NPQ associated with a lower rate of NPQ relaxation was observed in leaves infiltrated with KOX at pH 3.0, versus pH 7.0 (S2A Fig and S4 Movie). These observations confirm that the decrease in ambient pH is responsible for the NPQ increase. Furthermore, inhibition of electron transport with 3-(3,4-dichlorophenyl)-1,1-dimethylurea (DCMU) abolished the enhanced NPQ seen in Sclerotinia-inoculated leaves (S2B Fig), indicating that the Sclerotinia-induced NPQ increase requires photosynthetic electron transport that is presumably coupled with translocation of H+ from stroma to lumen to generate a trans-thylakoid proton gradient (ΔpH). In contrast, in the Sclerotinia-inoculated region, dissipation of the pH gradient using the uncoupler nigericin did not fully abolish the NPQ increase like in the control (S2C Fig). We then measured ATP synthase activity to indirectly reflect the changes of proton motive force. Treatment with KOX at pH 3.0 significantly attenuated ATP synthase activity, as represented by decreased inorganic phosphate (Pi) at 630 nm (S2D Fig). A down-regulated ATP synthase activity was also confirmed by a bioluminescent luciferase assay detecting ATP generation (S3 Fig). Taken together, these results suggest that the decreased ambient pH caused by Sclerotinia infection might down-regulate ATP synthase activity by limiting proton flux into the stroma and enhancing thylakoid lumen acidification under illumination, thus resulting in increased NPQ.
The components of zeaxanthin-related NPQ in Sclerotinia-infected leaves
Since lumen acidification is sensed by the PsbS protein during NPQ generation [19], we next measured NPQ in a Sclerotinia-infected PsbS mutant (npq4-1). As expected, defective PsbS function greatly attenuated the abnormal increase in NPQ induced by Sclerotinia (Fig 4A). NPQ was induced slowly to a total extent of only 0.3, and most of this NPQ failed to relax during the subsequent period in the dark, consistent with the known NPQ defect of this mutant [18].
In addition to PsbS protein, other factors, such as the violaxanthin de-epoxidase (VDE), are required for full activation of NPQ [26]. A mutant deficient in VDE, npq1-2, is compared with Col-0 wild-type after inoculation with Sclerotinia in Fig 4B. In the npq1-2 plant, Sclerotinia incubation did not induce increased NPQ, and the kinetic features consisted of a smaller increase and a slower second phase. After infiltration with dithiothreitol (DTT), a known inhibitor of VDE [16], NPQ formation was strongly inhibited in Sclerotinia-inoculated leaves (Fig 4C). Because VDE converts the carotenoid violaxanthin into zeaxanthin to participate in NPQ, we explored whether NPQ formation as associated with zeaxanthin level. Notably, Sclerotinia infection induced a high level of zeaxanthin-related NPQ (total NPQ kinetics minus NPQ kinetics + DTT [16,20]) (Fig 4D). Moreover, HPLC analysis showed that zeaxanthin increased 2.6-fold in Sclerotinia-infected Col-0 leaves compared to un-inoculated control leaves, with a corresponding decrease in violaxanthin content (Table 1). Conversely, presumably due to the loss of VDE, Sclerotinia infection did not promote greater zeaxanthin accumulation in the npq1-2 mutant. Moreover, associated with the conversion of most of the violaxanthin to zeaxanthin, one of violaxanthin’s catabolites, neoxanthin, also decreased in Sclerotinia-infected leaves (Table 1). Collectively, these results indicate that the Sclerotinia-induced NPQ increase was closely correlated with VDE-catalyzed zeaxanthin generation.
Table 1. Pigment composition of Sclerotinia-infected plants.
Vio | Ant | Zea | Neo | Lut | Chl a/b | |
---|---|---|---|---|---|---|
Col-0 | 3.1 ± 0.3 | 0.4 ± 0.1 | 0.8 ± 0.2 | 4.0 ± 0.2 | 14.1 ± 1.0 | 3.10 ± 0.12 |
Col-0+Sclerotinia | 0.9 ± 0.1 | 1.0± 0.2 | 2.2 ± 0.3 | 1.6 ± 0.6 | 13.6 ± 1.2 | 2.95 ± 0.06 |
npq1-2 | 3.2 ± 0.4 | ND | ND | 3.7 ± 0.4 | 14.0 ± 1.1 | 3.03 ± 0.10 |
npq1-2+Sclerotinia | 2.8 ± 0.5 | ND | ND | 3.5 ± 0.1 | 13.5 ± 0.5 | 2.93 ± 0.07 |
Four-week-old Arabidopsis leaves were inoculated with Sclerotinia for 3 h and kept under a light intensity of 130 μmol m-2 s-1. Xanthophylls were subjected to HPLC analysis after extraction with pre-cooled acetone. Pigment content was normalized to 100 Chl a+b molecules, except for Chl a/b. Abbreviations: Vio, violaxanthin; Ant, antheraxanthin; Zea, zeaxanthin; Neo, neoxanthin; Lut, lutein; ND, not detectable. Data shown are means ± SE (n = 3).
The decrease in the xanthophyll precursors antagonizes ABA biosynthesis and the subsequent resistance to Sclerotinia
Because xanthophyll precursors (i.e. violaxanthin, neoxanthin) play a key role in ABA biosynthesis [37,38], we explored whether changes in these precursors may affect ABA metabolism. qPCR results showed that expression of ABA biosynthesis genes, except for NCED3 (9-cis-epoxycarotenoid dioxygenases3), was not significantly affected after challenge with wild-type Sclerotinia or A2 mutant (Fig 5A). However, ABA immunoassays revealed that leaves incubated with the A2 mutant had elevated levels of ABA (Fig 5B), on average approximately 37% higher than controls (Fig 5C). In contrast, ABA levels in leaves inoculated with wild-type Sclerotinia were approximately 53% lower than those of control leaves (Fig 5C). In such circumstances, the expression of NCED3 may be increased in an attempt to compensate for limitations in ABA biosynthesis. It is worth mentioning that A2 mutant invasion always resulted in tissue yellowing surrounding the necrotic area (Fig 5D). Statistical analysis showed that the yellowing region accumulated a high level of ABA (Fig 5E). We next analyzed the impact of defective of VDE on ABA synthesis. After growth for four weeks in the greenhouse, the npq1-2 mutant showed similar ABA levels as Col-0. However, upon wild-type Sclerotinia infection, the mutation of VDE enzyme significantly suppressed the ABA levels decrease in the npq1-2 mutant (Fig 5F). These results suggest that Sclerotinia infection could regulate the VDE activity to modify ABA levels.
We then evaluated the efficiency of ABA in plant resistance to Sclerotinia. Upon Sclerotinia infection, the average necrotic lesions in leaves pretreated with ABA were significantly smaller than in water-pretreated plants. Likewise, the infected npq1-2 mutant showed a significant reduction in lesion area compared with Col-0, presumably due to the loss of VDE activity and associated maintenance of violaxanthin and/or neoxanthin levels and ABA synthesis (Fig 6A and 6B). However, due to defects in ABA sensing or ABA biosynthesis, the double mutants npq1-2/abi4-1 and npq1-2/aba2-3 were more susceptible to Sclerotinia than npq1-2 plants. Interestingly, treatment with ABA reverted the phenotype of the npq1-2/aba2-3 mutant but not the npq1-2/abi4-1 mutant (Fig 6C). This result is consistent with previous reports [60], suggesting that ABI4 is involved in the downstream signaling of ABA in plant resistance to Sclerotinia. Mutation of either the abi4 or the aba2 gene significantly increased the infectious ability of the A2 mutant in npq1-2/abi4-1 or npq1-2/aba2-3 plants (Fig 6D). Together, these results clearly indicate that Sclerotinia could manipulate the xanthophyll cycle and interfere with ABA biosynthesis and signaling to suppress host defense.
To gain further insight into the nature of ABA-induced resistance against Sclerotinia, we assessed changes in defense responses, including O2 - formation and callose deposition. As shown in Fig 6E, O2 - was detectable surrounding the A2 mutant-infected zone that were either sprayed or not with ABA. However, in the wild-type Sclerotinia-inoculated leaves, only pretreatment with ABA was able to induce a ring of O2 - accumulation at the periphery of the infection site (Figs 6E and S4A). Upon A2 mutant incubation, callose deposition was also observed in the leading edge of the necrotic regions. Similar results were obtained in the vicinity of wild-type Sclerotinia-induced necrotic lesions after ABA treatment (Figs 6F and S4B). Since the rate of oxalate diffusion in leaf tissue is correlated with plant susceptibility to Sclerotinia [66], we presumed that ABA-induced local reinforcement of the cell wall by forming callose might be an effective physical barrier to prevent the spread of oxalate and limit mycelial growth.
Discussion
The impact of NPQ on plant disease resistance
Light acts as an initial signal that activates the special photoreceptors (e.g., phytochromes, cryptochromes and phototropins) involved in different types of plant-pathogen interactions [6–7, 67]. In fact, the mechanisms that directly control photosynthetic light reactions also mediate important functions in plant response to pathogens [6, 68]. Recently, it has been reported that the light-induced reduction of the plastoquinone pool may trigger induction of defense-associated genes and the hypersensitive reaction [2, 69]. To manipulate such redox signals, pathogens may modulate the activation state of photoprotective mechanisms like changing the extent of NPQ, as an effective way to alter the redox status of the plastoquinone pool and generation of ROS from the photosynthetic electron transfer chain [68]. However, the impact on NPQ by different pathogens seems different, either increasing or decreasing NPQ [34–35]. At present, there is still no clear recognition of these pathogens’ role in manipulating NPQ. The measured NPQ under strong light is just as an indicator for early detection of pathogens in leaves [35,64]. Here, our results demonstrate for the first time that Sclerotinia infection induces a localized increase in NPQ in early pathogenesis under the natural and rather low growth light intensity (Figs 1 and 2). While there are a few reports of pathogens inducing NPQ under such low light intensity, not much is known about an involvement of this effect in the pathogenic process. The present data, however, revealed that an increased NPQ under such low light conditions caused changes in downstream cellular events, such as ABA biosynthesis and ROS generation, which weaken host defense responses during the natural pathogenic processes of Sclerotinia (Figs 5 and 6). Thus, the localized increase in NPQ in the early stage of infection cannot be regarded as a consequence of the metabolic perturbation of the host cell. Rather, this process is likely proactive in aiding pathogenic success. A more systematic study is required to validate this assumption.
Tissue acidification and zeaxanthin conversion are necessary for Sclerotinia-induced NPQ increase
Many pathogens are able to actively increase or decrease the surrounding pH at the infection site through alkalization or acidification [48–49]. For Sclerotinia, a low environmental pH may aid pathogenicity by affecting numerous pH-regulated genes and cell-wall-degrading enzymes [49–53]. As an early pathogenic event, the Sclerotinia-induced increase of NPQ demonstrated here in host plant is also closely related to a low ambient pH (Fig 3). Interestingly, incubation with another oxalate-secreting fungus, Botrytis cinerea, also induced an NPQ increase, although to a much smaller extent than that in Sclerotinia-inoculated regions (S5 Fig). Such differences might result from B. cinerea secreting lower amounts of oxalate than Sclerotinia [70]. However, for pathogens (e.g., Pseudomonas syringae) which cannot secrete acidic or alkaline factors, it is still unclear how they affect NPQ during their pathogenic progress [31–32]. NPQ increases or decreases in response to the level of light utilization in photosynthesis, and any impact of a pathogen on sugar export or sugar consumption is expected to result in changes in NPQ [12, 71]. In addition, NPQ is directly controlled by the trans-thylakoid proton gradient by at least two processes requiring a low lumenal pH, i.e., (i) the induction of VDE activity (and resulting conversion of violaxanthin to zeaxanthin) and (ii) the protonation of the PsbS protein leading to the engagement of zeaxanthin in the actual dissipation process [12,16–17,27]. It is noteworthy that the decrease in lumenal pH that induces NPQ does not have to be generated by photosynthetic electron transport [26,45,47]. Using isolated thylakoids, NPQ can be induced in darkness by simply lowering buffer pH [46]. While inhibition of linear electron flow with DCMU abolished the NPQ features induced by Sclerotinia, proton gradient collapse by treatment with the uncoupler nigericin did not fully abolish the Sclerotinia-induced NPQ increase (S2B and S2C Fig). Our data suggest that early Sclerotinia infection down-regulates ATP synthase activity and thereby leads to a decreased lumen pH and increased NPQ.
Furthermore, infected areas showed NPQ dynamics similar to those of aba1-3 (S6 Fig), a mutant deficient in the ZEP enzyme of the xanthophyll cycle that is associated with constitutive accumulation of zeaxanthin [20,72]. Consistent with the features of the latter mutant, our HPLC analyses of Col-0 leaves incubated with Sclerotinia revealed a significant increase in zeaxanthin content (Table 1). Accumulation of zeaxanthin is necessary to modulate the kinetics of NPQ, enhancing the rate of NPQ formation and retarding the rate of NPQ relaxation [72]. This effect can explain why inhibition of zeaxanthin formation abolished the Sclerotinia-induced NPQ increase in the npq1-2 mutant or wild-type leaves treated with DTT (Fig 5B and 5C).
Sclerotinia-induced modulation of the xanthophyll cycle curbs ABA biosynthesis
Biosynthesis of ABA begins inside the chloroplast and is limited by xanthoxin synthesized from violaxanthin [36–37,39]. In strong light, a low lumen pH activates VDE-catalyzed deepoxidation of violaxanthin to zeaxanthin [17,26]. Restraint of VDE activity results in violaxanthin accumulation and promotes ABA synthesis [4]. In the vtc1 mutant with a reduced level of the VDE substrate ascorbate, ABA content increased by 60% compared to that of wild-type [43]. Consequently, a reduction in ABA closely matched the decrease in the amounts of violaxanthin plus neoxanthin after infection with Sclerotinia (Table 1 and Fig 5). However, qPCR analysis showed that, except for NCED3, the expression of ABA biosynthesis genes was not significantly affected by wild-type Sclerotinia infection (Fig 5A). This suggests that, in the early stage of infection, regulation of ABA biosynthesis occurs primarily at the substrate level (violaxanthin) rather than at the transcriptional level. Since NCED3 is the key enzyme in the ABA biosynthesis pathway [39,73], the increase in NCED3 expression might result from the demand for ABA in the infected tissues. Sclerotinia infection generates the acidic environment that increases activation of VDE, promoting conversion of violaxanthin to zeaxanthin. The decrease in the ABA precursor violaxanthin may be the main reason for the reduced ABA levels in Sclerotinia-infected leaf discs. Taken together, our results suggest that modulation of the xanthophyll cycle provides a mechanism to adjust production of ABA for signaling purposes. To further evaluate this conclusion, it would be interesting to determine the interplay of lumen pH and/or sugar accumulation (and resulting NPQ changes) with ABA-mediated defense signaling in many other pathogens that can up-regulate or down-regulate NPQ in their pathogenic processes [32,34–35]. Additionally, it is worth mentioning that Sclerotinia infection caused stomatal pores to be more widely open within and around necrotic lesions after dark adaptation [59–60]. Because stomatal movement is tightly regulated by ABA-mediated signaling (such as ROS generation, Ca2+ permeable cation channels regulation) [74], decreased ABA levels might offer an explanation for the inhibitory action of Sclerotinia on stomatal closing.
Tissue defense responses induced by ABA participate in plant resistance to Sclerotinia
Although ABA’s role in influencing the outcome of plant-pathogen interactions is controversial, functional genetic studies have provided evidence for a positive role of ABA in defense against Sclerotinia [60–63]. In agreement with this view, exogenously applied ABA significantly restricted development of necrotic lesions caused by Sclerotinia. Importantly, the npq1-2 mutant showed more resistance to Sclerotinia compared with Col-0 plants (Fig 6A and 6B). It is likely that Sclerotinia cannot manipulate the xanthophyll cycle in npq1-2 plants due to their deficiency in the VDE enzyme, thus leading to unchanged ABA levels. This hypothesis was confirmed by measuring ABA levels in npq1-2 (Fig 5F). However, the defect in either ABA sensing or ABA biosynthesis weakened the resistance effect in npq1-2/abi4-1 or npq1-2/aba2-3 plants upon Sclerotinia infection (Fig 6C). The oxalate-deficient A2 mutant is less pathogenic than wild-type fungus [52]. Compared to wild-type Sclerotinia, the A2 mutant did not show significantly reduced susceptibility in npq1-2 (Fig 6D), which might result from the already higher levels of ABA induction in the plant response to A2 mutant infection (Fig 5B–5E). This could explain why the abi4 or aba2 mutations increased npq1-2 plant susceptibility to the A2 mutant (Fig 6D). Curiously, although silencing the NPQ machinery with mutant or inhibitor delayed the progression of lesion expansion, both wild-type Sclerotinia and the A2 mutant were still capable of infecting living plant tissue. One reason for this might be the use of PDA agar, which always leads to aggressive growth of Sclerotinia and overwhelms the defense capacity of plant. Actually, disease caused by this devastating necrotrophic fungal has traditionally been difficult to control [53]. Even if situated under unfavorable conditions, Sclerotinia could survive with the aid of sclerotia. Therefore, one can imagine that if the fungus is not directly killed at the source, it can breakthrough an already established defense system. Manipulation of NPQ in the pathogenic process of Sclerotinia is an early event, which primes other invasion processes like suppression of oxidative burst. Thus, we assume that the actual role of the Sclerotinia-induced increasing NPQ may contribute to successful early infection establishment.
ROS function as important second messengers in ABA-mediated defense signaling [75]. Manipulation of ROS signals in the pathogenic process of Sclerotinia is particularly intriguing. Sclerotinia-secreted oxalate initially suppressed host oxidative burst, but later promoted ROS generation to achieve pathogenic success [57–58]. Undoubtedly, inhibition of early ROS signaling can contribute to restraining plant activation of defense responses and favor of Sclerotinia invasion. At present, the physiological and molecular regulation mechanism of the initial ROS inhibition is not very clear. Although the previous research reported that the inhibitory effects of oxalate on ROS are largely independent of its acidity, lowering the medium pH indeed led to a greater inhibition of oxidative burst [57]. Tissue acidification is sufficient for Sclerotinia inducing an increase in NPQ, which is known to minimize production of 1O2* in the PSII antenna [15,26]. Moreover, NPQ is also correlated with the activation of photosynthetic control, which limits electron transport through the cytochrome b6f complex and alleviates the formation of ROS in PSI [68]. In addition to the effect of thermal dissipation (leading to NPQ) in causing de-excitation of singlet-excited chlorophyll, and thereby decreasing ROS formation, there is also a direct effect of zeaxanthin in deactivating ROS and their effect on biological membranes [33]. The Sclerotinia-induced increase in NPQ and in zeaxanthin accumulation was indeed paralleled by suppression of O2 - generation (Figs 1A–1E and 6E). In the early infection stage, there seems to be a correlation between the NPQ increase (and zeaxanthin accumulation) and oxidative burst inhibition. The Sclerotinia-induced increase of NPQ (and zeaxanthin accumulation) under low light should also be expected to attenuate ROS generated in the photosynthetic light reactions. In fact, there is a background level of triplet chlorophyll formation and potential singlet-oxygen formation even under low light level since the fraction of absorbed light converted to photosynthetic electron transport does not exceed about 85% [76]. It is worth noting that exogenous application of ABA reversed the decrease of O2 - (Fig 6E), possibly via activation of other cellular ROS-generating systems like NADPH oxidases. The latter mutations were showed susceptible to Sclerotinia in previous report [62]. Further studies are required to test this hypothesis.
In summary, our investigation provides evidence about an interplay of the xanthophyll cycle and plant resistance against the necrotrophic pathogen Sclerotinia. The possible correlations are summarized in the model presented in Fig 7. Initially, Sclerotinia secretes oxalate to acidify the infected tissues, which down-regulates ATP synthase activity and increases NPQ by protonating PsbS protein and activating the VDE enzyme. The latter goes on to convert violaxanthin to zeaxanthin via the intermediate antheraxanthin in the xanthophyll cycle. The decrease in precursor violaxanthin limits ABA biosynthesis and, in turn, affects tissue defense responses including ROS induction and callose deposition, which increase plant susceptibility to Sclerotinia. Additionally, the excellent works of Demmig-Adams & Adams group indicate that elevated NPQ and zeaxanthin accumulation have the potential to affect chloroplast redox status to lower oxidation-derived oxylipins (like jasmonic acid) formation [10–11,77], which may weaken callose formation and occlusion of sugar-loading complexes, presumably to facilitate pathogen spread via the phloem. In conclusion, the present study reveals a novel perspective on infection strategies of the necrotrophic fungal Sclerotinia, which provides a model of how photoprotective processes and metabolites are integrated into the plant defense network and thereby contributes to a better understanding of early plant-Sclerotinia interactions at the infection sites.
Materials and Methods
Plant material and chemicals treatment
Arabidopsis Columbia-0 (Col-0), abi4-1 (N8104), aba2-3 (N3834), npq1-2 (N3771) and npq4-1 (N66021) were obtained from the European Arabidopsis Stock Centre. For the generation of crosses npq1-2/abi4-1 and npq1-2/aba2-3, abi4-1 and aba2-3 mutants were directly crossed to npq1-2. F2 seeds were germinated on agar plates in the presence of 5 μM ABA. The seedlings with expanded cotyledons were screened via fluorescence video imaging (PAM-MINI, Walz, Germany). F3 lines were re-screened to identify true mutants, and F3 seedlings were used for experiments. Plants were cultivated in growth cabinets at 22°C with a 16-h photoperiod and a light intensity of 120 μmol photons m-2 s-1. The chemicals ABA, DTT and DCMU were purchased from Sigma-Aldrich; nigericin was obtained from J&K Scientific Ltd.. Detached leaves from 4-week-old plants were inoculated with Sclerotinia at 1 h after vacuum pre-infiltration with DCMU (8 μM), nigericin (50 μM) or DTT (10 μM), respectively. For ABA treatment, leaves were sprayed with 100 μM of cis, trans-ABA (dissolved in 0.1% (v/v) ethanol) at 24 h prior to Sclerotinia inoculation. Control leaves were sprayed with water containing 0.1% (v/v) ethanol.
Lesion area measurement
Wild-type Sclerotinia and an oxalate-deficient mutant (A2) were cultivated on potato dextrose agar at 21°C for 3 days. Agar plugs (diameter 0.3 or 0.8 cm) containing the leading edge of growing mycelia were used to inoculate leaves. Infected plants were kept under saturating humidity conditions in a clear plastic box. Photos of necrotic phenotype were captured by a numeric camera (HDR-XR500E, Sony). Lesion size was quantified in at least 10 leaves with a Carl Zeiss system as described by [59], with photographs captured by a Carl Zeiss AxioCam MRc5 camera installed on a Zeiss inverted microscope. Lesion area was quantified with the measurement tool ‘outline spline’ in AxioVision Rel.4.5 software. A measured example is given in S7 Fig.
Measurement of chlorophyll fluorescence parameters
Chlorophyll fluorescence parameters were measured with an Imaging-PAM Chlorophyll Fluorometer (PAM-MINI, Walz, Germany). The experimental procedures were as described previously [20, 32]. After inoculation with Sclerotinia, leaves were dark-adapted for 1 h prior to measurement. Parameters Fo (minimum fluorescence with PSII reaction centers fully open), Fm (maximum fluorescence after dark adaptation) and Fm’ (fluorescence level under actinic light-adapted state) were acquired by the ImagingWin software (ImagingWin v2.0m, Walz) (S8 Fig). A 0.8-s saturating pulse (4,000 μmol photons m-2 s-1) was applied to obtain Fm and Fm’. Fv/Fm and NPQ were automatically calculated by the ImagingWin software (Walz) using the formulas (Fm-Fo)/Fm and (Fm-Fm’)/Fm’, respectively. Actinic light of 725 μmol photons m-2 s-1 was selected as high light, and 133 μmol photons m-2 s-1 was used as low light. Images of the fluorescence parameters were displayed with a false color code, ranging from zero (black) to one (purple).
Investigation of the infection process by scanning electron microscope
After inoculated with Sclerotinia for 1h or 12h, the leaves were immediately fixed in formalin-acetic acid-alcohol for 24 h [78]. Samples were then washed three times in distilled water. Sections were next dehydrated through an ethanol series (70%, 80%, 90%, 95% and 100%; 30 min at each step). Ethanol-dehydrated samples were processed with critical point drying followed by platinum coating. Coated samples were scanned with a cold field scanning electron microscope at an accelerating voltage of 3.0 kV (S-4800, Hitachi).
Positional tissue acidification measurement
Positional pH was measured according to [65]. Sclerotinia-infected leaves were stained with LysoSensor Green DND-189 (2.5 μM) for 20 min or with acridine orange (50 μM) for 1.5 h. Stained leaves were washed twice with a washing buffer (10 mM KCl, 10 mM MES, pH 6.05). Fluorescence of DND-189 was acquired using a Zeiss LSM510 META system at excitation/ emission wavelengths of 458 nm/505 to 530 nm. Fluorescence emissions of acridine orange in red (615 to 660 nm) and green channels (505 to 550 nm) were obtained after excitation with 488 nm. Tissue acidification was represented by the ratio of the red-to-green emissions of acridine orange.
Qualitative measurement of ATP synthase activity
ATP synthase activity was assessed by determining the decrease in the concentration of inorganic phosphate (Pi) according to [79]. In brief, 10 mM KOX at a pH of 7.0 or 3.0 was incubated with 0.1 mg Chl ml-1 chloroplasts suspension (110 mM sorbitol and 17 mM Hepes-KOH, pH 8.0). After adding ADP (4 mM) and Pi (50 μM), chloroplasts were illuminated with 130 μmol photons m-2 s-1 for the indicated time (0–5 min) and stopped by addition of 4% (w/v) cold trichloroacetic acid. Samples were then mixed with 0.65 M sulfuric acid and 8.5 mM ammonium molybdate, followed by measuring absorbance at 630 nm (PerkinElmer, Lambda35, UK).
Pigment analysis
Sclerotinia-infected plants were kept under saturating humidity and a light intensity of 130 μmol m-2 s-1. Infected areas of leaves were obtained with a hole punch at 3 h after inoculation. Pigments were immediately extracted with pre-cooled acetone under dim light condition [80]. After filtering with a 0.2 μm filter, the extract was separated and quantified by HPLC with a Waters Spherisorb S5 ODS1 column (5.0 μm, 4.6 mm × 250 mm). The solvent system was according to Müller-Moulé et al. [81]. Solvent A (acetonitrile: methanol: Tris-HCl 0.1 M pH 8.0 [84: 2: 14]) was eluted with a linear gradient to 100% solvent B (methanol: ethyl acetate [68: 32]) within 15 min, followed by 5 min of solvent B. Relative contents were normalized to 100 chlorophyll a+b molecules.
Quantitative real-time PCR (qRT-PCR) analysis
Total RNA was extracted from Sclerotinia-infected zone using RNAiso Plus (Takara, Dalian, China) according to the supplier’s recommendation. First-strand cDNA was synthesized with the SuperScript II First-Strand Synthesis System (Invitrogen). qRT-PCR was performed using the lightCycler (Roche) real-time PCR detection system. Primer sequences (S1 Table) of ABA1 (At5g67030), ABA2 (At1g52340), ABA3 (At1g16540), NCED3 (At3g14440) and AAO3 (At2g27150) were used as described by [82]. Expression of target genes was normalized to ACTIN2.
Measurement of ABA
ABA extraction was according to [83]. Briefly, Sclerotinia-infected leaf discs were collected and frozen in liquid nitrogen. After grinding with a pre-chilled mortar and pestle on ice, the powder was extracted overnight at 4°C in a cold extraction buffer (80% methanol and 2% glacial acetic acid). The mixture was then centrifuged at 2,000 g for 5 min. The supernatant was run through a Sep-Pak C18 Plus Short Cartridge (Waters Corp) to remove polar compounds. ABA content was measured by a plant ABA ELISA Kit (Jiancheng, Nanjing, China).
Tissue immuno-localization of ABA was according to [84]. Sclerotinia-infected leaves were fixed overnight with 3% (W/V) para-formaldehyde in 4% (W/V) 1-ethyl-3-(3-dimethylaminopropyl) carbodiimide containing 0.1% (V/V) Triton X-100. Tissue cleaning was performed before infiltrating with wax. Sections (12 μm) were obtained with a sliding microtome (CM1850, Leica, Germany). After dewaxing and blocking, sections were incubated with rabbit anti-ABA primary antibody (Agrisera, Vännäs, Sweden) overnight. The fluorescence of Alexa 568 conjugated anti-rabbit secondary antibody was viewed with a confocal microscope (Zeiss LSM510 META).
Measurement of superoxide anion (O2 -) generation and callose deposition
Accumulation of O2 - was monitored in situ with nitroblue tetrazolium (NBT) as described previously [85]. Images were photographed using a Zeiss inverted microscope with a Carl Zeiss AxioCam MRc5 camera. Callose deposition was stained with 0.01% (w/v) aniline-blue and observed using a fluorescent microscope [86].
Supporting Information
Acknowledgments
We thank Prof. Martin B. Dickman (Texas A&M University, USA) for providing the strains of Sclerotinia sclerotiorum wild-type isolate (1980) and oxalate-deficient A2 mutant.
Data Availability
All relevant data are within the paper and its Supporting Information files.
Funding Statement
This research is supported by the Program for Changjiang Scholars and Innovative Research Team in University (IRT0829), the Key Program of NSFC-Guangdong Joint Funds of China (U0931005) and the National High Technology Research and Development Program of China (863 Program) (2007AA10Z204). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
References
- 1. Liu Y, Ren D, Pike S, Pallardy S, Gassmann W, et al. (2007) Chloroplast-generated reactive oxygen species are involved in hypersensitive response-like cell death mediated by a mitogen-activated protein kinase cascade. Plant J 51: 941–954. 10.1111/j.1365-313X.2007.03191.x . [DOI] [PubMed] [Google Scholar]
- 2. Mühlenbock P, Szechyńska-Hebda M, Płaszczyca M, Baudo M, Mateo A, et al. (2008) Chloroplast signaling and LESION SIMULATING DISEASE1 regulate crosstalk between light acclimation and immunity in Arabidopsis . Plant Cell 20: 2339–2356. 10.1105/tpc.108.059618 [DOI] [PMC free article] [PubMed] [Google Scholar]
- 3. Sierla M, Rahikainen M, Salojärvi J, Kangasjärvi J, Kangasjärvi S (2013) Apoplastic and chloroplastic redox signaling networks in plant stress responses. Antioxid Redox Signal 18: 2220–2239. 10.1089/ars.2012.5016 . [DOI] [PubMed] [Google Scholar]
- 4. Baier M, Dietz KJ (2005) Chloroplasts as source and target of cellular redox regulation, a discussion on chloroplast redox signals in the context of plant physiology. J Exp Bot 56: 1449–1462. 10.1093/jxb/eri161 . [DOI] [PubMed] [Google Scholar]
- 5. Berger S, Sinha AK, Roitsch T (2007) Plant physiology meets phytopathology, plant primary metabolism and plant-pathogen interactions. J Exp Bot 58: 4019–4026. 10.1093/jxb/erm298 . [DOI] [PubMed] [Google Scholar]
- 6. Kangasjärvi S, Neukermans J, Li S, Aro E, Noctor G (2012) Photosynthesis, photorespiration, and light signalling in defence responses. J Exp Bot 63: 1619–1636. 10.1093/jxb/err402 . [DOI] [PubMed] [Google Scholar]
- 7. Hua J (2013) Modulation of plant immunity by light, circadian rhythm, and temperature. Curr Opin Plant Biol 16: 406–413. 10.1016/j.pbi.2013.06.017 . [DOI] [PubMed] [Google Scholar]
- 8. Heiber I, Cai W, Baier M (2014) Linking chloroplast antioxidant defense to carbohydrate availability, the transcript abundance of stromal ascorbate peroxidase is sugar-controlled via ascorbate biosynthesis. Mol Plant 7: 58–70. 10.1093/mp/sst154 . [DOI] [PubMed] [Google Scholar]
- 9. Demmig-Adams B, Stewart JJ, Adams WW (2014) Multiple feedbacks between chloroplast and whole plant in the context of plant adaptation and acclimation to the environment. Philos T R Soc B 369: 20130244 10.1098/rstb.2013.0244 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 10. Demmig-Adams B, Cohu CM, Amiard V, Zadelhoff G, Veldink GA, et al. (2013) Emerging trade-offs—impact of photoprotectants (PsbS, xanthophylls, and vitamin E) on oxylipins as regulators of development and defense. New Phytol 197: 720–729. 10.1111/nph.12100 . [DOI] [PubMed] [Google Scholar]
- 11. Demmig-Adams B, Stewart JJ, Adams WW III (2014) Chloroplast photoprotection and the trade-off between abiotic and biotic defense In: Demmig-Adams B, Garab G, Adams WW III, Govindjee, editors. Non-photochemical quenching and energy dissipation in plants, algae and cyanobacteria. Springer; Netherlands: pp. 631–643. 10.1007/978-94-017-9032-1_28 [DOI] [Google Scholar]
- 12. Demmig-Adams B, Stewart JJ, Burch TA, Adams WW III (2014) Insights from placing photosynthetic light harvesting into context. J Phys Chem Lett 5: 2880–2889. 10.1021/jz5010768 [DOI] [PubMed] [Google Scholar]
- 13. Logan BA, Demmig-Adams B, Adams WW III, Bilger W (2014) Context, quantification, and measurement guide for non-photochemical quenching of chlorophyll fluorescence In: Demmig-Adams B, Garab G, Adams WW III, Govindjee, editors. Non-photochemical quenching and energy dissipation in plants, algae and cyanobacteria. Springer; Netherlands: pp. 187–201. 10.1007/978-94-017-9032-1_7 [DOI] [Google Scholar]
- 14. Horton P, Ruban AV (1992) Regulation of photosystem II. Photosynth Res 34: 375–385. 10.1007/BF00029812 . [DOI] [PubMed] [Google Scholar]
- 15. Horton P, Ruban AV, Walters RG (1996) Regulation of light harvesting in green plants. Annu Rev Plant Physiol Plant Mol Biol 47: 655–684. 10.1146/annurev.arplant.47.1.655 . [DOI] [PubMed] [Google Scholar]
- 16. Adams WW, Demmig-Adams B, Winter K (1990) Relative contributions of zeaxanthin-related and zeaxanthin-unrelated types of ‘high-energy state’ quenching of chlorophyll fluorescence in spinach leaves exposed to various environmental conditions. Plant Physiol 92: 302–309. 10.1104/pp.92.2.302 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 17. Demmig-Adams B, Adams WW (1996) The role of xanthophyll cycle carotenoids in the protection of photosynthesis. Trends Plant Sci 1: 21–26. 10.1016/S1360-1385(96)80019-7 [DOI] [Google Scholar]
- 18. Li XP, Björkman O, Shih C, Grossman AR, Rosenquist M, et al. (2000) A pigment-binding protein essential for regulation of photosynthetic light harvesting. Nature 403: 391–395. 10.1038/35000131 . [DOI] [PubMed] [Google Scholar]
- 19. Li XP, Gilmore AM, Caffari S, Bassi R, Golan T, et al. (2004) Regulation of photosynthetic light harvesting involves intrathylakoid lumen pH sensing by the PsbS protein. J Biol Chem 279: 22866–22874. 10.1074/jbc.M402461200 . [DOI] [PubMed] [Google Scholar]
- 20. Johnson MP, Pérez-Bueno ML, Zia A, Horton P, Ruban AV (2009) The zeaxanthin-independent and zeaxanthin-dependent qE components of nonphotochemical quenching involve common conformational changes within the photosystem II antenna in Arabidopsis . Plant Physiol 149: 1061–1075. 10.1104/pp.108.129957 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 21. Ruban AV, Johnson MP, Duffy CD (2012) The photoprotective molecular switch in the photosystem II antenna. Biochim Biophys Acta 1817: 167–181. 10.1016/j.bpj.2012.04.044 . [DOI] [PubMed] [Google Scholar]
- 22. Duffy CDP, Chmeliov J, Macernis M, Sulskus J, Valkunas L, et al. (2013) Modeling of fluorescence quenching by lutein in the plant light-harvesting complex LHCII. J Phys Chem B 117: 10974–10986. 10.1021/jp3110997 . [DOI] [PubMed] [Google Scholar]
- 23. Ilioaia C, Duffy CDP, Johnson MP, Ruban AV (2013) Changes in the energy transfer pathways within photosystem II antenna induced by xanthophyll cycle activity. J Phys Chem B 117: 5841–5847. 10.1021/jp402469d . [DOI] [PubMed] [Google Scholar]
- 24. Ruban AV, Walters RG, Horton P (1992) The molecular mechanism of the control of excitation energy dissipation in chloroplast membranes inhibition of ΔpH-dependent quenching of chlorophyll fluorescence by dicyclohexylcarbodiimide. FEBS Lett 309: 175–179. 10.1016/0014-5793(92)81089-5 . [DOI] [PubMed] [Google Scholar]
- 25. Crofts AR, Yerkes CT (1994) A molecular mechanism for qE quenching. FEBS Lett 352: 265–270. 10.1016/0014-5793(94)00976-7 . [DOI] [PubMed] [Google Scholar]
- 26. Müller P, Li XP, Niyogi KK (2001) Non-photochemical quenching. A response to excess light energy. Plant Physiol 125: 1558–1566. 10.1104/pp.125.4.1558 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 27. Demmig-Adams B, Cohu CM, Muller O, Adams WW III (2012) Modulation of photosynthetic energy conversion efficiency in nature: from seconds to seasons. Photosynth Res 113: 75–88. 10.1007/s11120-012-9761-6 . [DOI] [PubMed] [Google Scholar]
- 28. Frenkel M, Külheim C, Jänkänpää HJ, Skogström O, Dall’Osto L, et al. (2009) Improper excess light energy dissipation in Arabidopsis results in a metabolic reprogramming. BMC Plant Biol 9: 12 10.1186/1471-2229-9-12 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 29. Jänkänpää HJ, Frenkel M, Zulfugarov I, Reichelt M, Krieger-Liszkay A, et al. (2013) Non-photochemical quenching capacity in Arabidopsis thaliana affects herbivore behaviour. PloS ONE 8: e53232 10.1371/journal.pone.0053232 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 30. Göhre V, Jones AME, Sklenář J, Robatzek S, Weber APM (2012) Molecular crosstalk between PAMP-triggered immunity and photosynthesis. Mol Plant Microbe Interact 25: 1083–1092. 10.1094/MPMI-11-11-0301 . [DOI] [PubMed] [Google Scholar]
- 31. Berger S, Papadopoulos M, Schreiber U, Kaiser W, Roitsch T (2004) Complex regulation of gene expression, photosynthesis and sugar levels by pathogen infection in tomato. Physiol Plant 22: 419–428. 10.1111/j.1399-3054.2004.00433.x [DOI] [Google Scholar]
- 32. Bonfig KB, Schreiber U, Gabler A, Roitsch T, Berger S (2006) Infection with virulent and avirulent P. syringae strains differentially affects photosynthesis and sink metabolism in Arabidopsis leaves. Planta 225: 1–12. 10.1007/s00425-006-0303-3 . [DOI] [PubMed] [Google Scholar]
- 33. Havaux M, Niyogi KK (1999) The violaxanthin cycle protects plants from photooxidative damage by more than one mechanism. Proc Natl Acad Sci USA 96: 8762–8767. 10.1073/pnas.96.15.8762 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 34. Rodríguez-Moreno L, Pineda M, Soukupová J, Macho AP, Beuzón CR, et al. (2008) Early detection of bean infection by Pseudomonas syringae in asymptomatic leaf areas using chlorophyll fluorescence imaging. Photosynth Res 96: 27–35. 10.1007/s11120-007-9278-6 . [DOI] [PubMed] [Google Scholar]
- 35. Berger S, Benediktyova Z, Matous K, Bonfig K, Mueller MJ, et al. (2007) Visualization of dynamics of plant-pathogen interaction by novel combination of chlorophyll fluorescence imaging and statistical analysis, Differential effects of virulent and avirulent strains of P. syringae and of oxylipins on A. thaliana . J Exp Bot 58: 797–806. 10.1093/jxb/erl208 . [DOI] [PubMed] [Google Scholar]
- 36. Li Y, Walton DC (1990) Violaxanthin is an abscisic acid precursor in water-stressed dark-grown bean leaves. Plant Physiol 92: 551–559. 10.1104/pp.92.3.551 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 37. Seo M, Koshiba T (2002) Complex regulation of ABA biosynthesis in plants. Trends Plant Sci 7: 41–48. 10.1016/S1360-1385(01)02187-2 [DOI] [PubMed] [Google Scholar]
- 38. Wasilewska A, Vlad F, Sirichandra C, Redko Y, Jammes F, et al. (2008) An update on abscisic acid signaling in plants and more… Mol Plant 1: 198–217. 10.1093/mp/ssm022 . [DOI] [PubMed] [Google Scholar]
- 39. Milborrow BV (2001) The pathway of biosynthesis of abscisic acid in vascular plants, a review of the present state of knowledge of ABA biosynthesis. J Exp Bot 52: 1145–1164. 10.1093/jexbot/52.359.1145 . [DOI] [PubMed] [Google Scholar]
- 40. Duckham SC, Linforth RST, Taylor IB (1991) Abscisic-acid-deficient mutants at the aba gene locus of Arabidopsis thaliana are impaired in the epoxidation of zeaxanthin. Plant Cell Environ 14: 601–606. 10.1111/j.1365-3040.1991.tb01531.x [DOI] [Google Scholar]
- 41. Marin E, Nussaume L, Gonneau M, Sotta B, Hugueney P, et al. (1996) Molecular identification of zeaxanthin epoxidase of Nicotiana plumbaginifolia, a gene involved in abscisic acid biosynthesis and corresponding to the ABA locus of Arabidopsis thaliana . EMBO J 15: 2331–2342. . [PMC free article] [PubMed] [Google Scholar]
- 42. Bratt CE, Arvidsson PO, Carlsson M, Åkerlund HE (1995) Regulation of violaxanthin de-epoxidase activity by pH and ascorbate concentration. Photosynth Res 45: 169–175. 10.1007/BF00032588 . [DOI] [PubMed] [Google Scholar]
- 43. Pastori GM, Kiddle G, Antoniw J, Bernard S, Veljovic-Jovanovic S, et al. (2003) Leaf vitamin C contents modulate plant defense transcripts and regulate genes that control development through hormone signaling. Plant Cell 15: 939–951. 10.1105/tpc.010538 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 44. Zaks J, Amarnath K, Kramer DM, Niyogi KK, Fleming GR (2012) A kinetic model of rapidly reversible nonphotochemical quenching. Proc Natl Acad Sci USA 109: 15757–15762. 10.1073/pnas.1211017109 [DOI] [PMC free article] [PubMed] [Google Scholar]
- 45. Gilmore AM, Yamamoto HY (1992) Dark induction of zeaxanthin-dependent nonphotochemical fluorescence quenching mediated by ATP. Proc Natl Acad Sci USA 89: 1899–1903. 10.1073/pnas.89.5.1899 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 46. Krieger A, Moya I, Weis E (1992) Energy-dependent quenching of chlorophyll a fluorescence, effect of pH on stationary fluorescence and picosecond-relaxation kinetics in thylakoid membranes and photosystem II preparations. Biochim Biophys Acta 1102: 167–176. 10.1016/0005-2728(92)90097-L [DOI] [Google Scholar]
- 47. Demmig-Adams B, Gilmore AM, Adams W (1996) Carotenoids 3: in vivo function of carotenoids in higher plants. FASEB J 10: 403–412. 10.1096/fj.1530 . [DOI] [PubMed] [Google Scholar]
- 48. Criscitiello MF, Dickman MB, Samuel JE, de Figueiredo P (2013) Tripping on acid: trans-kingdom perspectives on biological acids in immunity and pathogenesis. PLoS Pathog 9: e1003402 10.1371/journal.ppat.1003402 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 49. Prusky D, Yakoby N (2003) Pathogenic fungi, leading or led by ambient pH? Mol Plant Pathol 4: 509–516. 10.1046/j.1364-3703.2003.00196.x . [DOI] [PubMed] [Google Scholar]
- 50. Rollins JA, Dickman MB (2001) pH signaling in Sclerotinia sclerotiorum, identification of a pacC/RIM1 homolog. App Environ Microb 67: 75–81. . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 51. Maxwell DP, Lumsden RD (1970) Oxalic acid production by Sclerotinia sclerotiorum in infected bean and in culture. Phytopathology 60: 1395–1398. 10.1094/Phyto-60-1395 [DOI] [Google Scholar]
- 52. Godoy G, Steadman JR, Dickman MB, Dam R (1990) Use of mutants to demonstrate the role of oxalic acid in pathogenicity of Sclerotinia sclerotiorum on Phaseolus vulgaris . Physiol Mol Plant Pathol 37: 179–191. 10.1016/0885-5765(90)90010-U [DOI] [Google Scholar]
- 53. Bolton MD, Thomma BP, Nelson BD (2006) Sclerotinia sclerotiorum (Lib.) de Bary: biology and molecular traits of a cosmopolitan pathogen. Mol Plant Pathol 7: 1–16. 10.1111/j.1364-3703.2005.00316.x . [DOI] [PubMed] [Google Scholar]
- 54. Errakhi R, Meimoun P, Lehner A, Vidal G, Briand J, et al. (2008) Anion channel activity is necessary to induce ethylene synthesis and programmed cell death in response to oxalic acid. J Exp Bot 59: 3121–3129. 10.1093/jxb/ern166 . [DOI] [PubMed] [Google Scholar]
- 55. Kim KS, Min JY, Dickman MB (2008) Oxalic acid is an elicitor of plant programmed cell death during Sclerotinia sclerotiorum disease development. Mol Plant Microbe Interact 21: 605–612. 10.1094/MPMI-21-5-0605 . [DOI] [PubMed] [Google Scholar]
- 56. Kabbage M, Williams B, Dickman MB (2013) Cell death control, the interplay of apoptosis and autophagy in the pathogenicity of Sclerotinia sclerotiorum . PLoS Patho 9: e1003287 10.1371/journal.ppat.1003287 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 57. Cessna SG, Sears VE, Dickman MB, Low PS (2000) Oxalic acid, a pathogenicity factor for Sclerotinia sclerotiorum, suppresses the oxidative burst of the host plant. Plant Cell 12: 2191–2199. 10.1105/tpc.12.11.2191 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 58. Williams B, Kabbage M, Kim HJ, Britt R, Dickman MB (2011) Tipping the balance: Sclerotinia sclerotiorum secreted oxalic acid suppresses host defenses by manipulating the host redox environment. PLoS Pathog 7: e1002107 10.1371/journal.ppat.1002107 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 59. Zhou J, Sun A, Xing D (2013) Modulation of cellular redox status by thiamine-activated NADPH oxidase confers Arabidopsis resistance to Sclerotinia sclerotiorum . J Exp Bot 64: 3261–3272. 10.1093/jxb/ert166 . [DOI] [PubMed] [Google Scholar]
- 60. Guimarães RL, Stotz HU (2004) Oxalate production by Sclerotinia sclerotiorum deregulates guard cells during infection. Plant Physiol 136: 3703–3711. 10.1104/pp.104.049650 [DOI] [PMC free article] [PubMed] [Google Scholar]
- 61. Guo XM, Stotz HU (2010) ABA signaling inhibits oxalate-induced production of reactive oxygen species and protects against Sclerotinia sclerotiorum in Arabidopsis thaliana . Eur J Plant Pathol 128: 7–19. 10.1007/s10658-010-9623-z [DOI] [Google Scholar]
- 62. Perchepied L, Balagué C, Riou C, Claudel-Renard C, Rivière N, et al. (2010) Nitric oxide participates in the complex interplay of defense-related signaling pathways controlling disease resistance to Sclerotinia sclerotiorum in Arabidopsis thaliana . Mol Plant Microbe Interact 23: 846–860. 10.1094/MPMI-23-7-0846 [DOI] [PubMed] [Google Scholar]
- 63. Stotz HU, Jikumaru Y, Shimada Y, Sasaki E, Stingl N, et al. (2011) Jasmonate-dependent and COI1-independent defense responses against Sclerotinia sclerotiorum in Arabidopsis thaliana: auxin is part of COI1-independent defense signaling. Plant Cell Physiol 52: 1941–1956. 10.1093/pcp/pcr127 . [DOI] [PubMed] [Google Scholar]
- 64. Murchie EH, Lawson T (2013) Chlorophyll fluorescence analysis: a guide to good practice and understanding some new applications. J Exp Bot 64:3983–3998. 10.1093/jxb/ert208 . [DOI] [PubMed] [Google Scholar]
- 65. Bak G, Lee EJ, Lee Y, Kato M, Segami S, et al. (2013) Rapid structural changes and acidification of guard cell vacuoles during stomatal closure require phosphatidylinositol 3, 5-bisphosphate. Plant Cell 25: 2202–2216. 10.1105/tpc.113.110411 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 66. Tu JC (1985) Tolerance of white bean (Phaseolus vulgaris) to white mold (Sclerotinia sclerotiorum) associated with tolerance to oxalic acid. Physiol Plant Pathol 26: 111–117. 10.1016/0048-4059(85)90034-7 [DOI] [Google Scholar]
- 67. Lau OS, Deng XW (2010) Plant hormone signaling lightens up: integrators of light and hormones. Curr Opin Plant Biol 13: 571–577. 10.1016/j.pbi.2010.07.001 . [DOI] [PubMed] [Google Scholar]
- 68. Kangasjärvi S, Tikkanen M, Durian G, Aro EM (2013) Photosynthetic light reactions-An adjustable hub in basic production and plant immunity signaling. Plant Physiol Bioch 81: 128–134. 10.1016/j.plaphy.2013.12.004 . [DOI] [PubMed] [Google Scholar]
- 69. Roden LC, Ingle RA (2009) Lights, rhythms, infection: the role of light and the circadian clock in determining the outcome of plant-pathogen interactions. Plant Cell 21: 2546–2552. 10.1105/tpc.109.069922 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 70. Manteau S, Abouna S, Lambert B, Legendre L (2003) Differential regulation by ambient pH of putative virulence factor secretion by the phytopathogenic fungus Botrytis cinerea . FEMS Microbiol Ecol 43: 359–366. 10.1111/j.1574-6941.2003.tb01076.x . [DOI] [PubMed] [Google Scholar]
- 71. Adams WW III, Muller O, Cohu CM, Demmig-Adams B (2013) May photoinhibition be a consequence, rather than a cause, of limited plant productivity? Photosynth Res 117: 31–44. 10.1007/s11120-013-9849-7 . [DOI] [PubMed] [Google Scholar]
- 72. Joliot PA, Finazzi G (2010) Proton equilibration in the chloroplast modulates multiphasic kinetics of nonphotochemical quenching of fluorescence in plants. Proc Natl Acad Sci USA 107: 12728–12733. 10.1073/pnas.1006399107 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 73. Xiong L, Zhu JK (2003) Regulation of abscisic acid biosynthesis. Plant Physiol 133: 29–36. 10.1104/pp.103.025395 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 74. Kwak JM, Mori IC, Pei ZM, Leonhardt N, et al. (2003) NADPH oxidase AtrbohD and AtrbohF genes function in ROS-dependent ABA signaling in Arabidopsis . EMBO J, 22: 2623–2633. 10.1093/emboj/cdg277 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 75. Torres MA, Dangl JL (2005) Functions of the respiratory burst oxidase in biotic interactions, abiotic stress and development. Curr Opin Plant Biol 8: 397–403. 10.1016/j.pbi.2005.05.014 . [DOI] [PubMed] [Google Scholar]
- 76. Demmig-Adams B, Adams WW III, Barker DH, Logan BA, Bowling DR, et al. (1996) Using chlorophyll fluorescence to assess the fraction of absorbed light allocated to thermal dissipation of excess excitation. Physiol Plantarum 98: 253–264. 10.1034/j.1399-3054.1996.980206.x [DOI] [Google Scholar]
- 77. Amiard V, Demmig-Adams B, Mueh KE, Turgeon R, Combs AF, et al. (2007) Role of light and jasmonic acid signaling in regulating foliar phloem cell wall ingrowth development. New Phytol 173: 772–731. 10.1111/j.1469-8137.2006.01954.x . [DOI] [PubMed] [Google Scholar]
- 78. Garg H, Li H, Sivasithamparam K, Kuo J, Barbetti MJ (2010) The infection processes of Sclerotinia sclerotiorum in cotyledon tissue of a resistant and a susceptible genotype of Brassica napus . Ann Bot 106: 897–908. 10.1093/aob/mcq196 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 79. Imashimizu M, Bernát G, Sunamura EI, Broekmans M, Konno H, et al. (2011) Regulation of F0F1-ATPase from Synechocystis sp. PCC 6803 by γ and ϵ subunits is significant for light/dark adaptation. J Biol Chem 286: 26595–26602. 10.1074/jbc.M111.234138 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 80. Thayer SS, Björkman O (1990) Leaf xanthophyll content and composition in sun and shade determined by HPLC. Photosynth Res 23: 331–343. 10.1007/BF00034864 [DOI] [PubMed] [Google Scholar]
- 81. Müller-Moulé P, Conklin PL, Niyogi KK (2002) Ascorbate deficiency can limit violaxanthin de-epoxidase activity in vivo. Plant Physiol 128: 970–977. 10.1104/pp.010924 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 82. Barrero J, Rodríguez PL, Quesada V, Piqueras P, Ponce MR, et al. (2006) Both abscisic acid (ABA)-dependent and ABA-independent pathways govern the induction of NCED3, AAO3 and ABA1 in response to salt stress. Plant Cell Environ 29: 2000–2008. 10.1111/j.1365-3040.2006.01576.x . [DOI] [PubMed] [Google Scholar]
- 83. Lin PC, Hwang SG, Endo A, Okamoto M, Koshiba T, et al. (2007) Ectopic expression of ABSCISIC ACID 2/GLUCOSE INSENSITIVE 1 in Arabidopsis promotes seed dormancy and stress tolerance. Plant physiol 143: 745–758. 10.1104/pp.106.084103 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 84. Schraut D, Ullrich CI, Hartung W (2004) Lateral ABA transport in maize roots (Zea mays): visualization by immunolocalization. J Exp Bot 55: 1635–1641. 10.1093/jxb/erh193 . [DOI] [PubMed] [Google Scholar]
- 85. Jabs T, Dietrich RA, Dangl JL (1996) Initiation of runaway cell death in an Arabidopsis mutant by extracellular superoxide. Science 273: 1853–1856. 10.1126/science.273.5283.1853 . [DOI] [PubMed] [Google Scholar]
- 86. Sun A, Nie S, Xing D (2012) Nitric oxide-mediated maintenance of redox homeostasis contributes to NPR1-dependent plant innate immunity triggered by lipopolysaccharides. Plant Physiol 160: 1081–1096. 10.1104/pp.112.201798 . [DOI] [PMC free article] [PubMed] [Google Scholar]
- 87. Wolf G, Fric F (1981) A rapid staining method for Erysiphe graminis f. sp. Hordei in and on whole barley leaves with a protein-specific dye. Phytopathology 71: 596–598. 10.1094/Phyto-71-596 [DOI] [Google Scholar]
Associated Data
This section collects any data citations, data availability statements, or supplementary materials included in this article.
Supplementary Materials
Data Availability Statement
All relevant data are within the paper and its Supporting Information files.