ABA Suppresses Botrytis cinerea Elicited NO Production in Tomato to Influence H2O2 Generation and Increase Host Susceptibility

Abscisic acid (ABA) production has emerged a susceptibility factor in plant-pathogen interactions. This work examined the interaction of ABA with nitric oxide (NO) in tomato following challenge with the ABA-synthesizing pathogen, Botrytis cinerea. Trace gas detection using a quantum cascade laser detected NO production within minutes of challenge with B. cinerea whilst photoacoustic laser detection detected ethylene production – an established mediator of defense against this pathogen – occurring after 6 h. Application of the NO generation inhibitor N-Nitro-L-arginine methyl ester (L-NAME) suppressed both NO and ethylene production and resistance against B. cinerea. The tomato mutant sitiens fails to accumulate ABA, shows increased resistance to B. cinerea and we noted exhibited elevated NO and ethylene production. Exogenous application of L-NAME or ABA reduced NO production in sitiens and reduced resistance to B. cinerea. Increased resistance to B. cinerea in sitiens have previously been linked to increased reactive oxygen species (ROS) generation but this was reduced in both L-NAME and ABA-treated sitiens. Taken together, our data suggests that ABA can decreases resistance to B. cinerea via reduction of NO production which also suppresses both ROS and ethylene production.


INTRODUCTION
The outcome of pathogen interactions with plants is governed by multiple events (reviewed by Jones and Dangl, 2006). Initial contact involves host detection of pathogen-associated molecular patterns [PAMPs, microbial-associated molecular patterns; also referred to as (MAMPs)] to initiate PAMPs-triggered immunity (PTI). Pathogens have evolved a range of effectors which can suppress PTI, some of which may be recognized by the host-classically by Resistance (R) genes -to initiate effector-triggered immunity (ETI) which can lead to the form of programmed cell death known as the hypersensitive response (HR; Mur et al., 2008). Superimposed on these interactions are the various pathogen-derived toxins, enzymes, and host modifying proteins that can drive symptom development. Based on disease symptoms it is possible to crudely classify pathogens into biotrophs (parasitizing living host tissue) or necrotrophs (predating death host tissue) or those exhibiting combinations of both lifestyles -hemibiotrophs (Schulze-Lefert and Panstruga, 2003;Oliver and Ipcho, 2004;Oliver and Solomon, 2010).
Pathogen-associated molecular patterns-triggered immunity and ETI-linked defense gene expression is co-ordinated by a large number of hormones (Robert-Seilaniantz et al., 2007). Traditionally, salicylic acid (SA) mediated defenses have been linked to defense against biotrophs and jasmonates (JA)/ethylene (Et) against necrotrophs (Oliver and Solomon, 2010) although this represents a considerable over-simplification (Robert-Seilaniantz et al., 2011). Nitric oxide (NO) should also be considered as a major defense initiator (Mur et al., 2013). Thus, NO has been shown to be rapidly generated in plants following challenge with biotrophic and necrotrophic pathogens (Delledonne et al., 1998;Foissner et al., 2000;Mur et al., 2005Mur et al., , 2012Prats et al., 2005;Besson-Bard et al., 2008). Despite many mechanisms of NO generation being proposed, it appears that under aerobic conditions NO is mostly produced by cytosolic nitrate reductase (NR) acting on NO − 2 as a nitrite reductase (Gupta et al., 2011). NO production has been linked to PTI, the HR and the formation of defense associated cell-wall appositions (Zeidler et al., 2004;Prats et al., 2005;Mur et al., 2008). Further, the importance of NO to plant defense has been shown through the use of chemical inhibitors, transgenic lines, or differential N fertilizer regimes to modify NO production and impact on the degree of resistance (Delledonne et al., 1998;Boccara et al., 2005;Mur et al., 2012;Gupta et al., 2013). The mechanisms through which NO impacts on defense signaling cascades have also been extensively examined, with reversible S-nitrosylation of proteins and irreversible tyrosine nitration of key components emerging as important regulatory events (Cecconi et al., 2009;Leitner et al., 2009). Notable examples of the role of S-nitrosylation in defense are the modification of the vital SA signaling component NON-EXPRESSOR OF PATHOGENESIS-RELATED PROTEIN1 (NPR1; Tada et al., 2008) and the reactive oxygen species (ROS) generating complex NADPH oxidase, AtRBOHD (Yun et al., 2011). Further, there is clear evidence that NO, ROS, and SA pathways work together to establish a systemic acquired resistance (SAR) that can be exhibited by the whole plants following the localized initiation of resistance (Wang et al., 2014). Such examples demonstrate the close interactive role of NO with other signaling pathways which also include JA and Et (Mur et al., 2013).
Abscisic acid (ABA) is classically associated with plant responses to abiotic stress particularly drought (Shinozaki and Yamaguchi Shinozaki, 1996) but is now well recognized to also play roles in plant responses to pathogens (Cao et al., 2011). However, rather than aiding resistance, ABA, appears to be mostly contributing to susceptibility. Thus, exogenous application of ABA increased the susceptibility of Arabidopsis to Pseudomonas syringae pv. tomato (Fan et al., 2009) or of rice to the rice blast pathogen Magnaporthe grisea; in this latter case even with avirulent strains (Jiang et al., 2010). Correspondingly, Arabidopsis ABA biosynthetic mutants exhibit enhanced resistance to P. syringae (de Torres-Zabala et al., 2007;Goritschnig et al., 2008). Considering mechanisms through which ABA antagonisms act, one mechanism appear to perturbation of SA signaling. Some key studies have shown that ABA suppresses expression of the SA biosynthetic gene ISOCHORISMATE SYNTHASE1 (ICS1) in Arabidopsis (Yasuda et al., 2008) and (e.g.) NPR1 in rice (Jiang et al., 2010). Other workers have shown a reciprocal antagonism with the increased disease resistance in the Arabidopsis mutant cpr22 at least partially linked to SA-mediated perturbation of ABA signaling Mosher et al., 2010). However, ABA impacts are not only associated with SA-mediated defenses -which are mostly deployed against biotrophs. ABA effects can also be seen in initiating ROS generation with latter contributing to ABA signaling (Pei et al., 2000). Similarly, ABA increase NO generation which can increase the activity of antioxidant enzymes (Zhou et al., 2005). Such observations suggest a subtle interaction between ABA, ROS, and NO.
Abscisic acid treatment could also compromise the resistance of Arabidopsis to the necrotroph B. cinerea (AbuQamar et al., 2006). Much work on the interaction of ABA and Botrytis has focused on the tomato mutant sitiens (Asselbergh et al., 2007). sitiens is deficient in ABA production through a mutation in the biosynthetic ABA-aldehyde oxidase (Harrison et al., 2011). sitiens exhibits considerably increased resistance to B. cinerea and this has been variously linked to increased SA effects (Audenaert et al., 2002) and/or epidermal hydrogen peroxide generation with cell wall modifications (Asselbergh et al., 2007). A similar link between ABA and suppression of ROS during attack by B. cinerea has been made in Arabidopsis (L' Haridon et al., 2011). Given such observations it is unsurprising that B. cinerea strains can encode genes for ABA biosynthesis (Gong et al., 2014).
In this current study, we examine the interaction between ABA and NO generation in tomato. Through the use of pharmacological inhibitors of NO generation we demonstrate the importance of NO to tomato defense against B. cinerea. Exploiting online, in planta measurements, we show a greatly elevated NO generation in the ABA deficient mutant sitiens. Suppression of NO production in sitiens, with NO generation inhibitors or the exogenous application of ABA, also compromised the increased resistance in this mutant to B. cinerea. Staining ROS production using 3,3 -diaminobenzidine (DAB) suggested that the levels were influenced by the rates of NO generation. We propose that ABA-influenced antagonism of NO generation could be an important mechanism through which pathogens can suppress defenses to establish compatible interactions with their host.

Tomato Plant Growth Conditions
Tomato genotypes, cv. Ailsa Craig and sitiens were obtained from the Tomato Genomics Resource Centre (TGRC) at UC, Davis USA 1 . Tomato plants were cultivated in Levington Universal compost in 10 cm diameter plastic pots. Plants were maintained in Conviron (Controlled Environments Ltd, UK) growth rooms at 24 • C with a light intensity of 110 µmol/m/s and a 12 h photoperiod for 4 weeks. At 4 weeks sitiens plants were considerably smaller than cv. Ailsa Craig but exhibited no evidence of any other defects (e.g., wilting) that were visible to the naked eye. Plants used for NO and Et measurements were transported to Radboud University (The Netherlands) via road and car ferry by the authors. Plants were then kept at Radboud University for 2 days under identical growth conditions to those in Aberystwyth to allow plant physiology to normalize prior to gas measurements being attempted.

Botrytis cinerea Culture and Storage
Botrytis cinerea (strain IMI 169558) was maintained on potato dextrose agar (PDA) in an inverted position in a Gallenkamp illuminated cooled incubator maintained at 20 • C with a 12 h photoperiod. PDA (Potato extract 4.0 g L −1 ; Glucose 20.0 g L −1 ; Agar 15.0 g L −1 ) was prepared according to manufacturer's instructions.
Conidia were harvested from the plate surface by flooding the plate with a carrier media of potato dextrose broth (PDB) and dislodging the conidia with an L-shaped glass rod. The density of conidia in the suspension was determined using a Neubauer Haemocytometer and the solution was diluted accordingly to 1 × 10 5 conidia mL −1 to provide a 30 mL standardized infection solution.
Four-week old tomato plants were inoculated with B. cinerea in one of two methods. Where trace gas detection (NO or Et) was being measured, the conidial suspension was sprayed on to plants to run-off. In all other occasions, inoculation involved application of 10 µL drops of spore solution, pipetted directly onto the adaxial leaf surface. Inoculation was made to the first four true leaves (excluding cotyledons), with seven drops of solution being applied to three leaflets per leaf with a total of 84 drops per plant.

Chemical Treatment of Tomato Plants
In wild type cv. Ailsa Craig plants, chemicals that would alter NO production were applied through the excised petioles of branches so that the entire compound leaf was treated. Selected compound leaves represented the oldest true leaves of 4-week-old plants. Excised branches were placed in 100 mL beakers with 50 mL of either 0.1 mM sodium nitroprusside (SNP, an NO donor) or 5 mM N-Nitro-L-arginine methyl ester (L-NAME; an inhibitor of NO generation) or N-Nitro-D-arginine methyl ester (D-NAME; a biologically inactive isomer of L-NAME) for 24 h prior to infecting the leaves with B. cinerea. Excised branches in beakers were maintained at 24 • C with a light intensity of 110 µmol/m/s and a 12 h photoperiod before and after spot-inoculation with B. cinerea.
Chemicals could not be applied to sitiens plants through cut petioles as this led to rapid tissue collapse of the leaves. Instead, chemicals were applied to intact 4-week-old sitiens plants as a foliar spray which included 0.2% Silwet (v/v) as wetting agent. Although this may not have allowed accurate estimations of applied dose to be determined it proved to be the only means (in our hands) to apply chemicals and maintain sitiens leaf viability.

Estimating Fungal Biomass by Quantitative PCR (qPCR)
DNA was extracted from eight leaf samples with single inoculations of B. cinerea using a DNeasy Mini Kit (Qiagen, UK) following manufacturer's instructions. DNA samples were diluted to 1 ng µL −1 ultrapure H 2 O. Samples (25 µL) were prepared by mixing 10 µL DNA solution with 16 µL SYBR TM Green Mastermix (Applied Biosystems, UK) and primers (300 nM) for Arabidopsis (iASK1: CTTATCGGATTTCTCTAT GTTTGGC; iASK2: GAGCTCCTGTTTATTTAACTTGTACA TACC) to generate an 131 bp amplicon and B. cinerea (CG11: AGCCTTATGTCCCTTCCCTTG; CG12: GAAGAG AAATGGAAAATGGTGAG) to generate a 58 bp amplicon (Gachon and Saindrenan, 2004). PCR used a Bio-Rad ABI7300 thermocycler amplifying using the following conditions: 15 min at 95 • C followed by 50 cycles of 95 • C for 15 s, 58 • C for 30 s and 72 • C for 1 min. This was followed by a dissociation (melting curve), according to the software procedure. Serial dilutions of pure genomic DNA from each species were used to trace a calibration curve, which was used to quantify plant and fungal DNA in each sample. Results were expressed as the CG11/iASK ratio of mock to inoculated samples.

Nitric Oxide (NO) Measurements Using a Quantum Cascade Laser-Based Sensor
The configuration of the quantum cascade laser (QCL)-based sensor for NO detection is detailed elsewhere (Cristescu et al., 2008). Briefly, the QCL emitting infrared light around 1900 cm −1 that passes through an absorption multi-pass cell, in which the airline enters transporting the NO released by a single inoculated rosette within a glass cuvette (∼500 mL volume). The NO production is directly detected by measuring the attenuation of the laser intensity due to the NO absorption in the cell. Infected plants were placed in glass cuvette and flushed with air at a controlled continuous flow rate of 1 L h −1 . Multiple cuvettes could be monitored in sequence, each being measured for ∼13 min. Each experiment was repeated to give similar results and the outcomes of one representative experiment are shown.

Ethylene Measurements Using Photoacoustic Laser Spectroscopy
Ethylene production was monitored in real-time using a gas flowthrough in-line system fitted with a photoacoustic laser-based ethylene detector (ETD-300, Sensor Sense BV) able to detect on-line 300 parts per trillion volume of ethylene within 5 s (Cristescu et al., 2008). Gas was regulated by an automated valve control box (VC-6, Sensor Sense B.V) and ethylene emanation from a tomato plant within a glass cuvette (254 mL volume) was alternately monitored for 15 min (5 s per acquisition point), at a controlled continuous flow rate of 1.5 L h −1 by flushing with air and preventing accumulation induced effects. KOH and CaCl 2 scrubbers were incorporated into the system to remove CO 2 and H 2 O, respectively. Each experiment was repeated to give similar results and the outcomes of one representative experiment are shown.

Visualization and Quantification of H 2 O 2 Generation
After sampling, the excised leaf disks were immersed in an aqueous solution of 1 mg ml −1 DAB (pH 3.8) and incubated at room temperature for 4 h. The leaves were removed from the DAB solution and fixed and cleared in absolute ethanol. The samples were scanned using a flat-bed scanner and the intensity of staining was quantified using Image-Quant TL, Software (GE Healthcare Life Sciences, UK).

Statistical Analyses
Data were subjected to analysis of variance using Minitab v.14 (Minitab Ltd, Coventry, UK), after which residual plots were inspected to confirm data conformed to normality. Comparisons of data points from different treatments with controls were performed using Tukey multiple pairwise comparison test. Timecourse data were compared using repeated measures anova. Differences with P < 0.05 were considered significant.

NO Production Is Tomato Is Required for Resistance to B. cinerea
We have demonstrated that NO contributes both to ethylene production and resistance to B. cinerea in Arabidopsis (Mur et al., 2012). To investigate the role of NO in tomato challenged with B. cinerea, the production of NO was measured using a QCLbased approach (Figure 1A). NO was rapidly produced in cv. Ailsa Craig following infection with B. cinerea even before it was possible -due to technical limitations -to take the first measurement at 0.5 h after inoculation. NO production was in slow decline over the subsequent 24 h period. This was specific to pathogen attack as application of PDB, used to resuspend the fungal conidia, failed to elicit increased NO production ( Figure 1A). Ethylene production was also elicited following challenge with B. cinerea but maximum rates of production were achieved some 6 h after that of NO ( Figure 1B).
To investigate the role of NO in contributing to resistance to B. cinerea experiments were undertaken when a NO donor (SNP) or an inhibitor of NO production (L-NAME) were applied to tomato plants. Thus, 0.1 mM SNP was applied to cut petioles of plants and after 24 h, inoculated with B. cinerea with lesion development assessed over a subsequent 72 h period. The developing B. cinerea lesions appeared to be smaller and more defined that those forming on controls at 72 h (compare Figures 2A,B). Conversely, if the 5 mM L-NAME -was applied to tomato leaves, B. cinerea lesions were highly variable in phenotype but were also larger than in control infections and occasionally coalesced to cover the entire leaf ( Figure 2C). If 5 mM D-NAME -an inactive isomer of L-NAME -was applied to the leaves, the B. cinerea lesions appeared to be more similar to those forming in control cv. Ailsa Craig plants (compare Figures 2D with 2A).
Measuring NO production in cv. Ailsa Craig and L-NAME-NAME fed plants suggested that the NO production was significantly (P < 0.001) reduced only in L-NAME-treated plants ( Figure 2E). Correspondingly, laser photoacoustic detection indicated that maximal ethylene production was seen following 9 hpi (hour after infection) was significantly (P < 0.001) reduced with L-NAME treatment ( Figure 2F). Taken together, these data suggest that NO, which may trigger ethylene production, contributes to tomato defense against B. cinerea.

The ABA Mutant Sitiens Displays High Level NO Production
We subsequently sought to test if NO played a role in the elevated resistance to B. cinerea which is exhibited by the  ABA-biosynthetic sitiens tomato mutant. Measuring B. cinerea elicited NO in sitiens showed >2-fold greater rates of production compared to cv. Ailsa Craig ( Figure 3A). The levels of NO produced in unchallenged sitiens plants did not significantly differ from those of cv. Ailsa Craig. B. cinerea-induced production of ethylene was also elevated in sitiens plants ( Figure 3B).
In order to establish the importance of increased NO in sitiens elevated resistance, cv. Ailsa Craig and sitiens plants were sprayed with L-NAME. The resulting lesions appeared to be form less quickly in L-NAME sprayed plants ( Figure 4A). Lesions forming on D-NAME treated plants did not appear different to the water treated control on either genotype (data not shown). To quantify the differences in lesion formation, B. cinerea fungal biomass was measured in lesions developing in cv. Ailsa Craig, sitiens and sitiens plants sprayed with either L-NAME or D-NAME at 72 hpi ( Figure 4B). This indicated reduced fungal development in sitiens which was consistent with the elevated resistance seen in this line. However, fungal biomass was significantly increased following L-NAME but not D-NAME, implicating NO as a component of cv. Ailsa Craig and; crucially, sitiens defense against B. cinerea. To confirm that that L-NAME was having an effect on NO production in sitiens, this was assessed at 6 hpi with B. cinerea in a parallel experiment. This a timepoint which has previously been indicated as the displaying maximal rates of NO production (Figures 1A and 3A). Spraying sitiens plants with L-NAME significantly (P < 0.01) decreased B. cinerea induced NO production compared to chemically untreated sitiens or D-NAME treated controls ( Figure 4C). Logistical constraints prevented the effects of L/D-NAME on NO production to be assessed in cv. Ailsa Craig.

ABA Suppresses B. cinerea NO and ROS Production
As sitiens is deficient in ABA, it was hypothesized that exogenous application of ABA could reduce NO production. Thus, sitiens plants as well as cv. Ailsa Craig were sprayed with 100 mM ABA and then after 1 h, we challenged with B. cinerea. Examining the effect of ABA treatment on lesion development in sitiens suggested that lesion sizes at 72 hpi tended to be greater compared to untreated controls. The phenotypic effects of ABA on cv. Ailsa Craig were more difficult to assess visually ( Figure 5A). This slight effect of ABA on B. cinerea infected on of cv. Ailsa Craig was also suggested from estimations of   . (B). B. cinerea fungal DNA content in 1 cm 2 diameter cored lesions isolated from 4 weeks old control cv. Ailsa Craig (AC), sitiens (SIT) sprayed 1 h prior to spot-inoculation with B. cinerea, sprayed with either L-NAME (L) or D-NAME (D; an inactive L-NAME isomer, 5 mM Nitro-d-arginine methyl ester) sampled at 72 h post-infection. Results are expressed as fold increase in biomass compared to t = 0 samples. Mean measurements (n = 5 cores) ±SE following inoculation within B. cinerea are given. Significant differences are indicated with letters. (C) NO production measured at 6 h (peak NO production; see Figure 1A) following spraying conidial suspensions of B. cinerea of whole 4 weeks old tomato sitiens plants. Three treatments were assessed; untreated sitiens plants (SIT), plants sprayed 24 h prior to inoculation with B. cinerea with either L-NAME (SIT-L-NAME) or D-NAME (SIT-D-NAME). Mean NO production was measured in three plants per treatment using a QCL system. Significant differences are indicated with letters. fungal biomass at 72 hpi ( Figure 5B). Although there was a trend toward increased fungal development with ABA treatment differences were not significant compared to controls. This was in contrast to sitiens where the application of ABA significantly increased fungal biomass suggesting that resistance was being reduced.
The impact on NO on ABA in sitiens was measured using the QCL-based system (Figure 5C). Logistical constraints limited the number of samples that could be measured so only the effect of ABA on sitiens was determined following challenge with B. cinerea. NO production in the control plant was in line with that previously observed (e.g., Figure 3A). However, rates of NO production were reduced by ∼half in two ABA treated sitiens plants (Figure 5C).
In a seminal paper, Asselbergh et al., (2007) linked resistance in sitiens to elevated H 2 O 2 production. We assessed if NO could also be contributing to H 2 O 2 generation in cv. Ailsa Craig and sitiens in cores from tomato leaves at 24 h after inoculation with B. cinerea and stained with DAB ( Figure 6A). Lesions with brown DAB staining were clearly observed in cv. Ailsa Craig and this appeared to be reduced by treatment with L-NAME and ABA. Greater staining was observed in sitiens compared to cv. Ailsa Craig and this was also reduced by L-NAME and ABA. This was further suggested when the extent of staining was measured using image analysis software ( Figure 6B). Although a semi-quantitative measure at best, the data suggested significant reductions (P < 0.01) in DAB we seen in L-NAME/ABA treated cv. Ailsa Craig and sitiens. In the case of treatments of sitiens L-NAME/ABA treated plants results in patterns of DAB staining that were not significantly different from similarly treated cv Ailsa Craig samples. The data suggested that NO contributes to the elicitation of B. cinerea elicited H 2 O 2 in wild type tomato and also to the elevated H 2 O 2 observed in sitiens.

DISCUSSION
Nitric oxide effects on plant responses to stress have been extensive characterized using Arabidopsis but not exclusively so, with some important studies being undertaken in tomato, which has the virtue of being a both a model species and an important crop. Examples of studies establishing NO effects in stress tolerance in tomato include resistance to bacterial wilt (caused by Ralstonia solanacearum; Hong et al., 2013), rootknot nematode (Meloidogyne incognita; Zhou et al., 2015), Cu and Cd  and heat shock (Piterkova et al., 2013). Our study sought to investigate further investigate role of NO in the interaction of tomato with B. cinerea. Resistance to B. cinerea in has been shown to be influenced by Et  Figures 1 and 2). The error bar represent the range of results around a mean (n = 2).   Robert-Seilaniantz et al., 2011) and we have demonstrated a link between NO and ethylene production in B. cinereachallenged Arabidopsis (Mur et al., 2012). We now sought to employ our on-line, in planta measurement platforms based on QCL detection and photoacoustic laser detection (Mur et al., 2011) to develop our understanding of the pathogenic interaction. NO production had already been reported in tomato cultures in response to B. cinerea and correlated with ROS generation, PCD and activity of the S-nitrosoglutathione modulating enzyme, S-nitrosoglutathione reductase (GSNOR; Pietrowska et al., 2015). Also, use of SNP has been shown to increase resistance to B. cinerea via mechanisms that, at least in part, were influences by MAPKinases (Zheng et al., 2014).
Our initial experiments demonstrated very rapid production (within 30 min) of NO following challenge with B. cinerea ( Figure 1A). These rapid induction kinetics are suggestive of responsiveness to PAMPs as described for chitosan from Fusarium eumartii (Terrile et al., 2015). Our use of L-NAME; (leaving aside doubts regarding its mechanism of action; Gupta et al., 2011) which may involve targeting NR (Rasul et al., 2012) suppressed NO production and lesion development establishing NO as a source of resistance in this pathosystem (Figure 2). How directly NO contributes to B. cinerea resistance needs to be clearly determined as L-NAME treated plants also displayed reduced Et production; an established mediator of defense against B. cinerea ( Figure 2F).
In considering how defense hormones act, many workers focus on how these act either singly or via interaction to increase resistance to a given pathogen or pathogens with a given infection strategy (Robert-Seilaniantz et al., 2007. Equally, ABA signaling has been shown to be "hijacked" by a range of pathogens to increase virulence (Grant et al., 2013). Delivery of effectors is a key feature of pathogen-focused suppression of host defenses and some effectors appear to target ABA signaling. The AvrB,AvrC effector domain from Xanthomonas campestris pv. campestris-induced NCED5, encoding a key enzyme of ABA biosynthesis, and increased ABA was important in disease development by this pathogen (Ho et al., 2013). There is some evidence that AvrPtoB can fulfill a similar role (de Torres-Zabala et al., 2007). Over-expression of AvrPtoB (also known as HopAB2) in transgenic plants induced the ABA biosynthetic gene NCED and ABA signaling focusing on abscisic acid insensitive 1 (ABI1) a protein phosphatases type 2C (PP2C). Alternatively, the Pseudomonas syringae effector HopAM1 enhances virulence via manipulation of sensitivity to ABA rather than initiating ABA biosynthesis (Goel et al., 2008). Moving beyond bacterial delivery of effectors, some fungal pathogen encode ABA biosynthetic genes and have been shown to synthesize ABA including Cercopsora, Fusarium, Rhizoctonia (reviewed by Cao et al., 2011), and of particular relevance to this current study, B. cinerea (Gong et al., 2014). Considering the mechanics of ABA promoted susceptibly, there is evidence that this causes reduced alterations in cell wall characteristics, ROS generation and callose deposition as well as defense gene expression (Asselbergh et al., 2007;de Torres-Zabala et al., 2007;Cao et al., 2011). Such wide ranging impact argues for multiple targets for ABA to confer increased susceptibility and paradigms from other systems; such as the phosphorylational regulation by ABA of the ROS generating NADPH oxidase AtrbohF in stomatal regulation, may be relevant (Sirichandra et al., 2009).
In order to provide a wider understanding of possible targets of ABA impacts on host responses we tested the possible interaction of ABA on NO effects. In undertaking this investigation we noted those few studies where ABA increases resistance (Ton and Mauch-Mani, 2004;Kaliff et al., 2007;De Vleesschauwer et al., 2010); thus as NO is key feature of both PTI and ETI (Mur et al., 2006) it was conceivable that ABA could increase NO generation. However, our analyses of the low ABA accumulating mutant sitiens, clearly indicated that ABA acted to suppress NO generation to promote virulence (Figure 4). This could implicate regulation of NR as a likely source of NO as a target for ABA manipulation. There is evidence for ABA acting via NR in Arabidopsis in the regulation of stomatal closure (Chen et al., 2015) and it is entirely conceivable that this is also the case in plant pathogen interactions. Thus, the regulation of NR by (for example) the phosphorylation of a conserved Ser residue or binding of 14-3-3 proteins could be targeted by ABA (Lillo et al., 2004). This stated it is important to unambiguously demonstrate that NR is the major source of NO in this B. cinerea -tomato interaction so that further work such as the use of RNAi or reduced NR activity lines is required. In this context, it should be noted that AtNOA1 although initially erroneously identified as a NO synthase (Guo et al., 2003), still contributes to NO -mediated events during plant responses to defense (Mandal et al., 2012). Indeed, although NOA1 was established as a mitochondria-located GTPase (Moreau et al., 2008) it appears to be regulating mitochondrial respiration (Heidler et al., 2011) which can be linked to NO production (Gas et al., 2009). Thus, modulation of NOA1 or mitochondrial function by ABA could be a target for ABA action. Indeed, ABA impact on certain mitochondrial GTPase and kinases (for example) have been noted Manara et al., 2016).
Increased resistance in ABA-deficient sitiens has been linked to elevated ROS production (Asselbergh et al., 2007) thus, the link between NO, ABA, and ROS was explored. Many studies have suggested that ROS generation is required to initiate NO production particularly in stomata (He et al., 2005;Lu et al., 2005;Bright et al., 2006;Shi et al., 2015). Additionally, ROS production was placed upstream of NO generation in the response of Pisum sativum to the PAMP, chitosan (Srivastava et al., 2009). Other authors have suggested that reduction of NO production through the use of NO scavengers or mutants resulted in increased ROS production (Tada et al., 2004;Asai et al., 2008) This could reflect a role for NO in modulating NADPH oxidase activity and this has been demonstrated by S-nitrosylation of AtrbohD (Asai et al., 2008;Yun et al., 2011). This could also reflect a role for NO as an ROS scavenger as suggested in early models (Beligni and Lamattina, 1999). In contrast, we demonstrated that the increase in ROS generation in response to B. cinerea in both sitiens and cv. Ailsa Craig could be reduced through the application of L-NAME (Figure 6). The placing of NO upstream of ROS generation was also suggested by Rasul et al. (2012) in oligogalacturonide-triggered immunity in Arabidopsis.
Taken together, such studies would suggest that the relative positioning of ROS and NO is context specific; possibly even pathogen-interaction specific. Our placing of NO upstream of ROS could suggest that two major elicitory defense signals could be suppressed via a single target, i.e., NR-mediated NO production (Figure 7).
Considering our observations together, we have revealed a new node for pathogen-mediated suppression of host defenses, namely, NO generation. If NO is derived from NR activity, this would implicate either NR activity itself and/or N − 3 N −

AUTHOR CONTRIBUTIONS
AS, AA, JM, and LM produced the data used in this manuscript. AS carried out the estimations of fungal virulence based on fungal DNA content, H 2 O 2 measurements, infections of different tomato genotypes. AA also contributed to estimations of fungal virulence based on fungal DNA content. JM and LM undertook the measurements of NO and ethylene. NO and ethylene measurements were supervised by SC and FH. Overall project supervision and direction was provided by LM. The manuscript was written by LM, FH, and SC.

FUNDING
The work described in this manuscript was partially supported by the EU Human Resources Mobility Fund and the Nigerian Tertiary Education Trust (TET) Fund.