Abstract
Abiotic and biotic stress factors are the major constrains for the realization of crop yield potential. As climate change progresses, the spread and intensity of abiotic as well as biotic stressors is expected to increase, with increased probability of crops being exposed to both types of stress. Shielding crops from combinatorial stress requires a better understanding of the plant’s response and its genetic architecture. In this study, we evaluated resistance to salt stress, powdery mildew and to both stresses combined in tomato, using the Solanum habrochaites LYC4 introgression line (IL) population. The IL population segregated for both salt stress tolerance and powdery mildew resistance. Using SNP array marker data, QTLs were identified for salt tolerance as well as Na+ and Cl− accumulation. Salt stress increased the susceptibility of the population to powdery mildew in an additive manner. Phenotypic variation for disease resistance was reduced under combined stress as indicated by the coefficient of variation. No correlation was found between disease resistance and Na+ and Cl− accumulation under combined stress Most genetic loci were specific for either salt stress tolerance or powdery mildew resistance. These findings increase our understanding of the genetic regulation of responses to abiotic and biotic stress combinations and can provide leads to more efficiently breeding tomatoes and other crops with a high level of disease resistance while maintaining their performance in combination with abiotic stress.
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Introduction
Crops grown in open fields encounter multiple unfavorable conditions for optimal plant growth and yield, of both abiotic and biotic origin. The ongoing climate change, accelerated by the increase in atmospheric CO2 concentration (Peters et al. 2011), is resulting in an average rise in temperature and decrease in precipitation especially in regions with temperate climates (Dai 2013), which further intensifies agricultural land deterioration due to extended periods of drought and an increase in soil salinity (Munns and Tester 2008; Zhao and Running 2010). Moreover, an increase in temperature and ambient CO2 concentration could directly influence plant pathogens spread and geographic distribution. While studies show that on many occasions the effects on pathogenicity are pathosystem-specific (Coakley et al. 1999), the consensus is that elevated temperatures will result in pathogen geographic expansion and enhanced fecundity, increasing the chances for host range expansion and rise of more virulent strains (Garrett et al. 2006; Harvell et al. 2002). As predictions point to increased possibilities of plants encountering abiotic and/or biotic stress, exposure to combined stresses is expected to become more frequent.
The limited data available for plant responses under abiotic and biotic stress combinations point to predominantly negative interactions at the phenotypic level (Mittler 2006; Kissoudis et al. 2014). Increased soil salt concentration results in enhanced susceptibility to soil borne diseases in tomato (Triky-Dotan et al. 2005) and other crop species (Al-Sadi et al. 2010; You et al. 2011), and similar trends are observed under water deficit (Jordan et al. 1984). Observations of the effects of abiotic stress on foliar pathogens are on the other hand mixed, with studies reporting either enhanced (Achuo et al. 2006; Wiese et al. 2004), or decreased resistance (Roubtsova and Bostock 2009; Sanogo 2004). Abiotic stress severity can affect responses to abiotic and biotic stress combinations (Soliman and Kostandi 1998), and therefore the outcome of the interaction may be dependent on the specific environmental conditions under which it occurs.
Indications for stress regulatory crosstalk can be found at the phenotypic level, and are evident as well at the gene expression level (Kissoudis et al. 2014). Recently, the transcriptome of Arabidopsis subjected to combinations of various abiotic and biotic stressors was analyzed (Atkinson et al. 2013; Prasch and Sonnewald 2013; Rasmussen et al. 2013). The striking commonality of all these studies is the unique responses observed under stress combinations that could not be predicted by the response to individual stressors. Moreover it was observed that the response of a significant number of transcripts was cancelled or prioritized under stress combinations in comparison with the individual stress, suggesting antagonistic interactions with potential detrimental effects on plant adaptation under combined stress.
Apart from the characterization of individual genes involved in both abiotic and biotic stress (Asano et al. 2012; Ramírez et al. 2009) and the recent reports on transcriptomic characterization of the response to various stress combinations in Arabidopsis, the genetic architecture of plant response to combinatorial stress has not been investigated.
In this paper we study the interaction between salinity stress and powdery mildew (PM) infection in tomato. Tomato (Solanum lycopersicum L.) possesses unique properties, as it is both an economically important crop, the first vegetable in production in the world (FAOSTAT 2011), and a model plant species, due to its diploid, relatively compact, and recently sequenced genome (Sato et al. 2012) and its large genetic and genomic resources (Ranjan et al. 2012). Tomato productivity is affected by a high incidence of increased soil salinity in the areas of cultivation (Cuartero et al. 2006). Additionally, fungal pathogens can significantly limit productivity by colonizing the foliage or the fruits. The biotrophic ascomycete Oidium neolycopersici (causing PM) is one of the economically most important foliar pathogens of tomato, both in the greenhouse and in open field conditions (Jones et al. 2001).
We evaluated a Solanum habrochaites introgression line (IL) population (accession LYC4 as the donor) in the background of cultivated tomato (cv. Moneymaker, Finkers et al. 2007b) for our study. S. habrochaites is native to high altitude habitats in the Andean mountains (Grandillo et al. 2011), and various accessions were used as a source for cold tolerance (Venema et al. 2008) and resistance to a wide range of fungal pathogens (Grandillo et al. 2011) including PM (Huang et al. 2000). The LYC4 population was evaluated previously for Botrytis resistance (Finkers et al. 2007b) and parthenocarpy (Gorguet et al. 2008).
The results presented in this paper show that the LYC4 IL population segregated for both salt stress tolerance and PM resistance. QTLs conferring resistance to the individual stresses were identified using a high density SNP array for accurate localisation of introgressions. In addition the effect of salt stress on the genetic factors involved in PM resistance was evaluated. Various new genetic loci contributing to tomato salt stress tolerance and PM resistance were discovered. Salt stress increased susceptibility to PM, reducing phenotypic variation for disease resistance. These results provide novel genetic resources for enhancing salt stress tolerance and PM resistance in tomato and enhance our understanding for plant responses under abiotic and biotic stress combinations.
Materials and methods
Plant material
The core collection of a S. habrochaites LYC4 introgression line (IL) population in the genetic background of S. lycopersicum cv. Moneymaker (MM), consisting of 31 ILs covering most of the tomato genome, was used in this study (Finkers et al. 2007b). The population was originally generated aiming at maximum coverage of the wild species genome and parts of each chromosome being present in at least three ILs as assessed with AFLP markers. Twenty-nine of the ILs were genotyped using a custom made single nucleotide polymorphism (SNP) Infinium array containing 5,528 SNPs, as described by (Víquez-Zamora et al. 2013). The introgressed regions according to the SNP data were visualized using the software Graphical GenoTypes 2 (Van Berloo 2008).
Experimental conditions and treatments
Experiments were carried out in the Unifarm greenhouse facilities of Wageningen University & Research Centre. The photoperiod regime was 16 h light and 8 h dark. Greenhouse air humidity was 70 %. Additional lighting (100 Wm−2) was used if the incoming shortwave radiation was below 200 Wm−2.
Tomato seeds were sown in peat and transplanted to 3L pots filled with vermiculite. The plantlets were irrigated with half strength Hoagland’s nutrient solution every 2 days initially, and every day in the final week of the experiment. Due to spatial restrictions and PM containment measures the simultaneous assessment of all four treatments was not possible, therefore, two subsequent and partially overlapping experiments were carried out. In the first experiment, salt stress was applied to the population by the addition of 100 mM NaCl to the nutrient solution of 3 weeks-old plants (5 plants per line), for 21 days. The pots were watered until leaching, to ensure uniformity of the treatment and to prevent NaCl accumulation. The concentration of NaCl in the pots was regularly monitored by measuring the electrical conductivity (EC) of the leachate after the completion of the irrigation.
In the second experiment, PM and combined salt stress-PM resistance were assessed as follows: 3-week old plants (4 plants per line) were watered with a solution containing 100 mM NaCl for 1 week. Subsequently, PM was applied to both (4-week old) salt stressed and non-salt stressed plants according to (Bai et al. 2003) by spraying a suspension of 5 × 104 conidia.ml−1 [prepared by washing conidial spores from leaves of heavily infected (sporulation stage) MM plants]. The plants were grown for another 2 weeks after inoculation.
Traits measured
Salt stress experiment
Chlorophyll content was measured using a SPAD-502 meter (Minolta, Osaka, Japan) at the third and fourth leaf counting from the bottom, 1 day before harvest. Plant height and shoot fresh weight (FW) were recorded at the end of the experiment. Dry weight was determined after drying the plant tissues in a forced-air oven at 70 °C until the samples reached stable weight. Salt tolerance index was calculated as the ratio of (fresh or dry) shoot biomass under salt stress and biomass under control conditions for each genotype.
Powdery mildew and combined stress experiment
The disease severity was expressed as disease index (DI), assessed at 12 dpi (days post inoculation). DI was expressed on a scale from 0 to 5, slightly modified from (Bai et al. 2003), to increase the resolution of infection incidence in order to obtain a more quantitative measure of disease resistance. The values corresponded to macroscopic observations of PM growth and sporulation where 0 = healthy plant, no visible sporulation, 1 = <0.1–10 % of foliar area affected, slight sporulation, 2 = 10–20 % area affected, 3 = 20–30 % area affected, 4 = 30–50 % area affected and 5 = >50 % area affected with abundant sporulation.
Ion chromatography
For the ion content determination the oven-dried leaves of tomato plants were ground to fine powder using a hammer mill with 1 mm sieve. The powder was ashed at 575 °C for 6 h. Ashed samples were dissolved by shaking for 15 min in 1 ml 3 M formic acid at 99 °C and then diluted with 9 ml MilliQ water. A final 500× dilution was subsequently prepared by mixing 0.2 ml sample solution with 9.8 ml MilliQ water. The concentration of Na+, K+, Ca2+, Mg2+ and Cl−, \({\text{PO}}_{4}^{3 - }\) and \({\text{SO}}_{4}^{2 - }\) of each sample was measured using ion chromatography (IC) system 850 Professional (Metrohm Switzerland). The anions were determined using Metrosap A 150, 150/4.0 mm column equipped with a Metrosap C5/5 Supp 4/6 Guard column and the cations with Metrosap C4 Supp 4, 250/4.0 mm column equipped with a Metrosap A Supp 4/6 Guard column.
Statistical and bioinformatics analyses
Experiments were carried out in a Split plot design with five replications for the salinity stress experiments and four replications for the PM and combined stress experiment. Statistical analyses were performed using Genstat 15th edition. Introgression lines with trait values significantly different from the recurrent parent (MM) were identified using a two-sided Dunnett test (Dunnett 1955) at a type I error rate of α = 0.05, and the underlying introgression was assigned as a QTL. Correlations between traits were calculated using the Pearson correlation coefficient (p ≤ 0.05). The Coefficient of Variation \(\left( {{\text{CV}} = {\text{s}}/\overline{\text{x}} \times 100} \right)\) was used to estimate trait phenotypic variation of the population. The discovered QTLs were surveyed for underlying candidate genes with Marker2Sequence software (Chibon et al. 2012) using as input the position of the distal-most SNP markers of the S. habrochaites LYC4 introgressed region.
Results
Genotyping of ILs
The custom made, Illumina Infinium based array described in (Víquez-Zamora et al. 2013) was used for the genotyping of the S. habrochaites LYC4 ILs. 1,508 SNPs out of 5,528 (27.2 %) were polymorphic between the S. lycopersicum and S. habrochaites LYC4 parental lines after SNP filtering with the quality control criteria (Víquez-Zamora et al. 2013, Supp. Table 1). The markers were landmarked on the genomic sequence of tomato (Víquez-Zamora et al. 2013), which facilitated precise localization of the introgressions of interest and subsequent investigation of underlying putative candidate genes located in the introgressed regions. As expected the size of the introgressions in many occasions deviated significantly on what was predicted by the genetic distances examined previously with AFLP markers (Finkers et al. 2007b). On some occasions (such as in ILs 2–3 and 8–2) introgression were revealed in different chromosomes compared to the ones originally assigned (Supp. Table 1; Supp. Fig. 1). However as these are only a handful of exceptions we maintained the naming of the lines of the population as reported previously (Finkers et al. 2007b).
Variation in phenotypic traits
Solanum habrochaites LYC4 (LYC4) was selected from different tomato wild species and tomato breeding lines that were evaluated for salt tolerance and powdery mildew (PM) resistance. LYC4 exhibited significantly higher salt Tolerance index (calculated as the ratio of total above ground FW under salinity stress and that under control conditions, expressed as percentage, 74.2 % compared to 56.5 % of MM), and was highly resistant to PM (DI score of 0.7 compared to 4 of MM). Therefore, the S. habrochaites LYC4 IL population in the background of S. lycopersicum cv. MM as described in (Finkers et al. 2007b) was chosen for this study.
The frequency distribution of the population growth (total above ground fresh biomass) under non-stress conditions revealed a normal distribution (Shapiro–Wilk test, p = 0.903) after excluding LYC4, which had significantly lower biomass than the population (Fig. 1a). Similarly, relative FW under salt stress (salt tolerance index-see below) followed a normal distribution (Shapiro–Wilk test, p = 0.267) (Fig. 1b). Interestingly, the majority of the population exhibited increased salt stress tolerance compared to the recurrent parent (MM).
On the other hand, the disease index (DI) frequency distribution deviated from normality, exhibiting negative skewness. This was due to the majority of the individuals of the population being susceptible to PM, and none exhibiting the level of resistance of the donor parent LYC4 (Fig. 1c). DI frequency distribution under combined salt stress and PM was similarly negatively skewed, but with an increased degree of skewness indicating that salt stress further enhanced disease susceptibility (Fig. 1d).
Identification of QTLs for salt tolerance and ion accumulation
FW and DW under salt stress were highly correlated (r = 0.9, p < 0.0001), however variation between ILs was more pronounced for FW. Therefore, salt tolerance index was determined as ratio of total above ground FW under salinity and FW under control conditions expressed as percentage, normalizing the differences in growth of the different genotypes under control conditions.
Ten ILs (IL1-2, IL1-4, IL2-3, IL3-2, IL4-2, IL8-2, IL9-1, IL10-2, IL10-3, IL10-4) exhibited higher salt tolerance index compared to the recurrent parent MM (Dunnett test, p < 0.05, Fig. 2a, Table 1). Salt tolerance of those lines ranged from 67 to 80 % maintenance of growth under saline conditions compared to 56.5 % of MM, with IL8-2 exhibiting the highest degree of tolerance. Among those lines, IL2-3 and IL3-2 additionally exhibited significantly higher FW compared to the recurrent parent under salt stress (108.7 and 113.2 g, respectively, compared to 89 g for MM).
Putative QTLs for salt tolerance reside in the introgressed regions of the salt tolerant lines. Several lines carried large introgressions, covering almost complete chromosomes (e.g. ILs 2-3, 3-2 and 8-2), and therefore pinpointing underlying candidate genes from the numerous genes in these introgressions is not possible. Shared introgressions between different ILs conferring salt tolerance provides a strong and more precise indication for a QTL. Both ILs 1-4 and 9-1 carried a ~4 Mbp introgression at the top of Chr. 9, while a common overlapping region of ~2.7 Mbp at the bottom of Chr. 10 was shared between ILs 10-2, 10-3 and 10-4.
As ion toxicity in the shoot is an important aspect of salt stress, the population was profiled for ion concentrations in shoots under both control and salt stress conditions. The genetic effects of introgressions on variation in concentrations of the macronutrients Na+, Cl−, K+, Ca2+, Mg2+, \({\text{PO}}_{4}^{3 - }\) and \({\text{SO}}_{4}^{2 - }\) and the consequences for salt tolerance and DI were investigated (Table 2). No significant differences in ion concentrations were identified between the ILs and MM under control conditions. Under salt stress, introgression lines IL12-1 and IL12-3 accumulated significantly less Na+ compared to MM (18.2 and 18.6 compared to 25.5 mg/g dry biomass respectively, Table 1). IL12-3 was not genotyped with the SNP array, however using the AFLP data from Finkers et al. (2007b), the introgressed region was shown to overlap with that of IL12-1. Therefore a common genetic factor potentially underlies the reduced Na+ accumulation in those lines. IL8-2 and IL12-3 accumulated significantly less Cl− compared to MM (30.1 and 28.2 compared to 41.6 mg/g dry biomass respectively). K+ concentration was significantly higher in IL9-1 (33.0 compared to 25.2 mg/g dry biomass in MM). K+/Na+ ratio, considered to be an indicator for salt tolerance (Shabala and Cuin 2008), was significantly increased in the lines IL2-3, IL6-3, IL9-1, IL12-3 and IL12-1 compared to MM. Finally, except for \({\text{SO}}_{4}^{2 - }\) in IL3-1 which exhibited a significantly higher content−, Ca2+, Mg2+ and \({\text{PO}}_{4}^{3 - }\) concentrations were not significantly different in any of the ILs under salt stress.
Correlation analyses
Correlation analysis (Pearson r, p < 0.05) under control conditions revealed a positive correlation between FW and \({\text{SO}}_{4}^{2 - }\) concentration (r = 0.61) and a negative correlation with \({\text{PO}}_{4}^{3 - }\) concentration (r = −0.43). Under salt stress only a few significant correlations were observed (Supp. Table 2). Growth under salt stress was correlated with growth under non-stress conditions, however the degree of correlation (r = 0.7, p < 0.001) suggests a considerable differential effect of salt stress on growth, supported by the statistically significant interaction observed between FW and stress levels in an ANOVA analysis (p < 0.001). Relative growth under salt stress was strongly negatively correlated with growth under non-stressed conditions (r = −0.54, p = 0.0015), indicating that large plants on average are less tolerant to salt stress than smaller plants. Relative growth under salt stress was not correlated with any of the ions measured, except for Na+ for which a weak positive correlation was observed (r = 0.37, p = 0.039).
QTLs for powdery mildew resistance
Solanum habrochaites LYC4 exhibited a high level of resistance against PM, with limited disease symptoms (no HR observed). Several introgression lines (IL3-2, IL4-2, IL4-3, IL6-2, IL9-1 and IL12-3) had increased resistance compared to MM, however they were considerably more susceptible than LYC4 (mean DI range 2.2–3.0 compared to 4.0 for MM and 0.7 for LYC4, Figs. 2b, 3, Table 1). Partial resistance in IL3-2, which carries an introgression covering a large part of Chromosome 3, was characterized by the development of necrotic (HR-like) lesions at the site of fungal spore development. All other lines exhibited quantitative resistance with no visible cell death. IL4-3 and IL9-1 both carry a ~4 Mbp introgression at the top of Chr. 9. However, IL4-3 has an additional introgression at Chr. 4 that overlaps for ~3 Mbp with the introgressed segment of IL4-2, a line that was also more resistant. IL6-2 carries two introgressions of ~2.7 and 4.8 Mbp on chromosomes 6 and 7, respectively. The AFLP marker data point to a large introgression in IL12-3 at the bottom arm of Chr. 12.
Correlation analysis of DI with growth and ion content revealed a positive correlation with FW (r = 0.47, p = 0.006) and a negative with \({\text{PO}}_{4}^{3 - }\) content (r = −0.31, p = 0.047), while no significant correlation was observed between DI and chlorophyll content.
Combined salt and PM stresses
Salt stress imposition significantly increased the susceptibility to PM of the population (mean DI of 4.45 compared to 3.65 without salt stress, p < 0.001). The effect was more pronounced when only the lines with significantly greater resistance than MM under either stress condition were included (ILs 3-2, 4-2, 4-3, 6-2, 9-1, 10-1 and 12-3, mean DI of 3.93 compared to 2.78 without salt stress, p < 0.001).
Three out of four ILs identified with significantly reduced DI under combined stress conditions (ILs 4-2, 4-3 and 9-1) had also significantly reduced DI under non-salt stress conditions (Figs. 2c, 3; Table 1). Only IL10-1 exhibited increased resistance to PM uniquely under salt stress; it was only marginally (non-significantly) more resistant than MM under non-salt stress conditions.
To evaluate the effect of combinatorial stress on the phenotypic variation of the population for PM resistance, the coefficient of variation (CV) values for DI were compared under PM and combined PM and salt stress. The CV under the combination of stresses was considerably lower than under PM infection (12.63 % compared to 18.92 %), which might indicate that the phenotypic variation for PM was reduced under salt stress (Fig. 4a). This could also be a result of the population susceptibility shifting towards the maximum of the disease score scale. However, when CV was calculated for the lines that were more resistant under either conditions a similar trend was observed (14.53 %, mean = 3.93 (combined stress) compared to 18.56 %, mean = 2.78 (PM only), Fig. 4b).
No significant differences were observed between the ILs and MM for ion content under combined salt stress and therefore no QTLs could be assigned.
DI in non-salt stressed plants was significantly correlated with DI under combined stress (r = 0.77, p < 0.0001, Fig. 5), suggesting minor interaction of salt stress with the genotypic differences in plant susceptibility, supported by the (marginally) non-significant (p = 0.092) interaction observed, after ANOVA analysis. No further significant correlations were identified under combined stress, except a weak positive correlation of DI with chlorophyll content (r = 0.32).
Discussion
Salt stress and powdery mildew individually pose a significant threat to tomato production, and the probability of these occurring at the same time may result in non-additive effects on plant fitness. Therefore we examined the responses of the S. habrochaites LYC4 IL population to both separately applied salt stress and PM and the combination of these stresses. Even though the experiments were done in the greenhouse in a controlled environment, small differences in the environmental conditions between both experiments that influence the plants’ performance and the measurements could not be avoided. Therefore, direct comparisons of the trait values measured in the two different experiments need to be done with caution. Nevertheless, QTL co-localization will be discussed, as most of the QTLs identified were reproducible in subsequent experiments with the selected ILs.
S. habrochaites LYC4 carries significant variation for tolerance and ion homeostasis under salt stress
Several S. habrochaites introgressions contributed significantly to salt tolerance, and our results indicate that under the stress conditions applied the IL lines that were larger in size were more affected by salt stress. The more vigorous (or high yielding) genotypes under non-stress conditions are often also the best-performing plants under mild stress in particular, with usually no crossover interactions (Blum 2005). The salt concentration applied in our experiments (100 mM NaCl) is considered to exceed this crossover point for tomato (Maggio et al. 2007). This is supported by the significant interactions between plant biomass and salinity level and the moderate correlation between plant biomass under control and salt stress conditions. Interestingly, two ILs with higher FW than the recurrent parent MM under both control and salt stress (IL3-2 and 2-3) also exhibited a higher salt tolerance index. These properties make them valuable starting material for salt tolerance breeding, especially IL2-3 which was previously shown to out-yield, under control conditions, the parental line MM while IL3-2 had substantially lower fruit yields (Finkers 2007).
Several genomic regions of LYC4 contributed to an increased salt tolerance index. Many of the QTLs identified in this study co-localized with previously discovered stress tolerance-contributing loci in segregating populations derived from crosses with wild tomato species (Table 1). The introgressed region in Chr. 1 of IL2-3 coincides with QTLs identified in previous studies for enhanced germination, vegetative growth and fruit yield under salt stress (Foolad 1999; Villalta et al. 2007). In this region, many candidate genes reside that are involved in the regulation of ion homeostasis, such as NHX3, NHX4 and SOS1 (Gálvez et al. 2012; OlÍas et al. 2009), and for redox homeostasis such as Cu/ZnSOD1 (Chen et al. 2009). Notably, IL2-3 exhibited lower Na+ accumulation (19.9 mg/g compared to 25.5 mg/g dry biomass of MM), but it was marginally below the significance cut-off level and therefore no QTL was assigned. An introgressed segment from Chr. 7 present in IL8-2 had the strongest association with salt tolerance index. Two HKT genes were recently found to reside on Chr. 7, potentially being causal for a QTL controlling Na+ and K+ concentration (Asins et al. 2013). However the introgression of IL8-2 covers almost the whole Chr.7, so linking it with the HKT function should be done with caution. IL8-2 also exhibited significantly lower Cl− accumulation, which was shown to contribute to salt tolerance in barley (Tavakkoli et al. 2011).
The introgressed segments on chromosomes 9, 10 and 12 found in the IL set used for this study are relatively small. IL9-1 exhibited higher levels of K+, as well as higher K/Na ratio compared to MM under salt stress. A putative potassium channel, and cyclic nucleotide gated channels involved in K+ transport (Shabala and Cuin 2008) reside in the introgressed region of this line as well as other genes involved in plant stress responses. (Table 1). The introgressed region on Chr. 10 contains ethylene response factors (ERFs) involved in stress tolerance and growth regulation under abiotic stress (Cheng et al. 2013; Dubois et al. 2013) as well as aquaporins, GSTs and RLKs.
No correlation was found between salt tolerance index and ion content, except for Na+ accumulation, which was weakly positively correlated. The lack of correlation is evidenced by the limited co-localization of QTLs for salt tolerance index and ion content (Supp. Table 4), as well as the insignificant contribution to salt tolerance of a shared introgression in Chr. 12, resulting in lower Na+ accumulation, carried by ILs 12-1 and 12-3. The type and the size of the population may have limited the discovery of correlations, as usually unique introgressions are present in the different ILs, which despite the possibility of co-regulating different traits, is present in only a few individuals of the population, resulting in non-statistically significant associations. However previous studies have as well identified a non-significant correlation of Na+ accumulation with salt stress tolerance in tomato (Rao et al. 2013; Villalta et al. 2008). In fact, Na+ can be used as an osmoticum facilitating water status maintenance, as it was observed in S. pimpinellifolium (Bolarin et al. 2001). and this is reflected as well in our results where LYC4 is more tolerant compared to MM despite having higher Na+ accumulation, suggesting that Na+ tissue tolerance (by storing Na+ in the vacuole or older leaves) contributes to LYC4 salt tolerance. On the other hand the lack of co-localization between many salt tolerance and ion content QTLs, offers the opportunity to combine them through pyramiding and examine epistatic interactions that additionally affect salt tolerance.
S. habrochaites LYC4 introgression contribute to partial resistance to powdery mildew
Solanum habrochaites LYC4 exhibited a high level of resistance to PM. None of the introgression lines exhibited the same level of resistance. This phenomenon was also observed in a previous study of this IL population on resistance to Botrytis cinerea (Finkers et al. 2007b). It can be either a result of incomplete representation of the wild species genome in the IL population, or the breakdown of epistatic interactions between loci, which are common in plant defense signaling (Alcázar et al. 2009). Resistance to PM in LYC4 is not the result of HR. In addition LYC4 was previously found to be resistant to various pathogens and insects (Finkers et al. 2007a; Yu et al. 2010). Therefore increased basal resistance, or secretion of secondary metabolites (antibiosis) and leaf surface structure such as the trichomes (antixenosis), may contribute to resistance (Nonomura et al. 2009), which should be further examined in this population.
Introgressions conferring PM resistance do not coincide with previously identified regions with PM resistance genes (Li et al. 2007, 2012). All previously identified genes confer strong resistance to PM, in contrast to the QTLs reported here. Because of the size of the introgressions, no specific genes can be pinpointed for increased resistance, though several candidate genes are present (Table 1), on many occasions (such as the RLKs) in multiple copies.
Salinity stress has a negative impact on powdery mildew resistance
Salt stress (100 mM) increased PM susceptibility in all genotypes of the population. This is in agreement with the majority of studies in literature reporting a suppressive effect of abiotic stress on defense responses and increase in susceptibility. In Arabidopsis thaliana abiotic stressors were shown to suppress various aspects of the defense response. Salt stress inhibited salicylic acid (SA) biosynthesis and the induction of systemic acquired resistance (Yasuda et al. 2008), while drought and heat stress suppressed basal and R-gene mediated resistance against a virus (Prasch and Sonnewald 2013). Contrarily, a previous study in tomato reported a weak positive effect of salt stress (100 mM) on PM resistance (Achuo et al. 2006). These observations can be a result of the longer period the plants experienced salt stress (14 days vs 7 in our study), which may have allowed a buildup of Na+ and Cl− concentration to toxic for the fungus levels We have observed a significant positive impact of Na+ and Cl− accumulation on powdery mildew resistance in experiments with varied salt stress levels, with mild salt stress increasing susceptibility while stronger salt stress is reversing the effect (unpublished results).
Powdery mildew resistance QTLs were fewer under combined salt stress than under only PM stress alone but they were mostly shared between the two treatments. This result, in conjunction with the high correlation of DI between both conditions, indicates that salinity stress had a general suppressive effect on the defense response rather than a specific interaction. Observations from molecular studies further support this conclusion, as several components of the defense signaling network appear to be down-regulated under abiotic stress (Mang et al. 2012; Prasch and Sonnewald 2013). Both the fewer QTLs identified as well the reduced phenotypic variability of PM resistance under combined stress point to a negative impact of salt stress on the expression of genotypic variation under these conditions, potentially altering the adaptive potential/fitness. Phenotypic plasticity is considered pivotal in the plant’s ability to adapt to changing environments (Ghalambor et al. 2007; Nicotra et al. 2010), and a reduction of this phenotypic plasticity when exposed to multiple stresses can have additional detrimental effects on plants and crop productivity. Moreover, it highlights an additional aspect that may pose a challenge for breeding for resistance to combined stresses: reduction in phenotypic variation can negatively affect selection efficiency when resistance is partial or quantitatively controlled. On the other hand selection for increased resistance under combined stress can be more robust when resistance is controlled by a single (or few) R-genes as it can quickly eliminate R-genes that become non functional under these conditions.
Na+ and Cl− accumulation under salt stress can have a harmful effect on both the host and the pathogen (Blomberg and Adler 1993). However, no significant correlation between disease severity and Na+ and Cl− accumulation was found in our study. It is possible that the concentration of NaCl applied did not result in the accumulation of Na+ and Cl− up to levels that were toxic for the fungus (evidenced by the increased fungal growth under salt stress). The severity of the stress can influence the magnitude of impact of another stress (Soliman and Kostandi 1998). Preliminary results in our laboratory indicated that the impact of salt stress on PM growth may depend on the severity of the applied stress (unpublished results). The lack of correlation of internal salt accumulation with PM growth may therefore be explained by relatively low (subtoxic) levels of Na+ and Cl Alternatively, the genetic variability in the population for Na+ and Cl− accumulation and/or disease resistance may be too limited, as evidenced by the small number of QTLs identified under salt stress alone and none under stress combination. In addition, the weak positive correlation between DI and chlorophyll content may point to the significance of nutrient availability for fungal growth, and could be indicative of the negative interaction between salt tolerance and disease under combined stress. Salt tolerance is often characterized by delayed senescence and the maintenance of chlorophyll, a nitrogenous compound, under stress can positively interact with pathogen growth by facilitating (biotrophic) pathogen nutrition (Walters and Bingham 2007).
Our data point to distinct genetic architectures for salt stress tolerance and PM resistance in the LYC4 IL population, with few QTLs shared (Supp. Table 3) and no significant correlations observed. The shared QTLs are relatively large, with possibly different genes being responsible for resistance to either stress. The introgression of IL9-1 (resistant under all stress conditions), may contribute to multiple stress tolerance. Although there are genes present in the introgressed region that have a clear function in pathogen response and resistance (RLKs, PRs, PAL), there are also multiple genes encoding TFs, redox and ethylene signaling components that have broad functions in stress responses. Therefore, further dissection of multiple and combined stress tolerance in IL9-1 is needed, using different approaches such as fine mapping, transcriptomics analyses and reverse genetics.
In conclusion, several genomic regions were identified in the S. habrochaites LYC4 IL population that can contribute to salt stress tolerance and PM resistance in tomato. Salt stress predisposed plants towards increased susceptibility to PM. The reduction in phenotypic variation under stress combination may have additional implications on plant and crop performance and breeding efforts. As no correlation was observed between salt stress tolerance and PM resistance, the different components appear to not interact with each other. Therefore a strategy of combining resistance and tolerance traits may be successful. With the availability of the tomato genome sequence and high throughput phenotypic analyses, phenotypic responses and tolerance to stress combination can be precisely associated with the genotype and breeding of combinatorial stress resilient crops may be feasible.
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Christos Kissoudis is supported by “Alexander S. Onassis” Public Benefit Foundation scholarship.
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Supplementary Fig. 1 Graphical genotypes of the S. habrochaites LYC4 ILs and the parental lines (colour codes are similar to Fig. 1) (JPEG 254 kb)
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Supplementary Table 1 Position of the polymorphic SNP markers between MM and S. habrochaites LYC4 on the tomato reference genome sequence (ITAG2.3 release) and the genomic localization of introgressions carried by the S. habrochaites LYC4 ILs (XLSX 248 kb)
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Supplementary Table 2 Pearson correlation analysis between growth traits and mineral element content under salt stress. Significant correlations are highlighted (XLSX 13 kb)
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Supplementary Table 3 Overview of LYC4 ILs exhibiting significant differences compared to MM under salt stress, powdery mildew infection and their combination (marked with “x”, ion content traits are under salt stress only). ILs with increased tolerance to all three stress conditions compared to MM are highlighted (DOCX 17 kb)
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Kissoudis, C., Chowdhury, R., van Heusden, S. et al. Combined biotic and abiotic stress resistance in tomato. Euphytica 202, 317–332 (2015). https://doi.org/10.1007/s10681-015-1363-x
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DOI: https://doi.org/10.1007/s10681-015-1363-x