Next Article in Journal
Thermo Condition Determines the Uptake of Autumn and Winter Applied Nitrogen and Subsequent Utilization in Spring Tea (Camellia sinensis L.)
Next Article in Special Issue
Deciphering Resistance to Root-Knot Nematodes in Prunus for Rootstock Breeding: Sources, Genetics and Characterization of the Ma Locus
Previous Article in Journal
Stevia rebaudiana Bertoni: The Interaction of Night Interruption on Gas Exchange, Flowering Delay, and Steviol Glycosides Synthesis
Previous Article in Special Issue
Water Use Efficiency and Nutritional Status of a New Grapevine Rootstock Selection
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Horticulturae
Volume 7
Issue 12
10.3390/horticulturae7120542
horticulturae-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles thumb_up
...
Endorse textsms
...
Comment
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Article

Effective Categorization of Tolerance to Salt Stress through Clustering Prunus Rootstocks According to Their Physiological Performances

by
Guillermo Toro
1,
Paula Pimentel
1 and
Ariel Salvatierra
2,*
1
Laboratorio de Fisiología del Estrés, Centro de Estudios Avanzados en Fruticultura (CEAF), Camino Las Parcelas 882, km 105 Ruta 5 Sur, Sector Los Choapinos, Rengo 2940000, Chile
2
Laboratorio de Genómica Vegetal, Centro de Estudios Avanzados en Fruticultura (CEAF), Camino Las Parcelas 882, km 105 Ruta 5 Sur, Sector Los Choapinos, Rengo 2940000, Chile
*
Author to whom correspondence should be addressed.
Horticulturae 2021, 7(12), 542; https://doi.org/10.3390/horticulturae7120542
Submission received: 31 October 2021 / Revised: 27 November 2021 / Accepted: 30 November 2021 / Published: 2 December 2021
(This article belongs to the Special Issue Rootstock Genetics and Improvement in Breeding)
Browse Figures
Versions Notes

Abstract

:
The effects of climate change on traditional stone fruit producing areas, together with the generation of new varieties with lower chilling requirements that allow the cultivation of previously unexplored areas, are setting up a challenging scenario for the establishment of productive orchards that must be more efficient in their capacity to adapt to new edaphoclimatic conditions. In this context, the rootstock breeding programs are a key piece in the agronomic strategy to achieve this adaptation through the development of rootstocks compatible with the new varieties and capable of transferring their tolerance to stress. An effective categorization of phenotypes within the germplasm involved in a plant breeding program is of utmost importance. Through the measurement of physiological parameters in both roots and leaves, tolerance to saline stress (120 mM NaCl) was evaluated in seven Prunus rootstocks whose genetic background included representatives of the subgenera Prunus, Cerasus, and Amygdalus. To group the genotypes according to their physiological performance under salt stress, an agglomerative hierarchical clustering was applied. The genotypes were grouped into three clusters containing rootstocks very sensitive (‘Mazzard F12/1’), moderately tolerant (‘Maxma 60’, ‘Cab6P’ and ‘AGAF 0204-09’), and tolerant (‘Mariana 2624’, ‘Garnem’ and ‘Colt’) to salt stress. ‘Mariana 2624’, a plum-based rootstock, was identified as the most tolerant Prunus rootstock. The information reported is valuable both in the productive context, for the selection of the most appropriate rootstocks to establish an orchard, and in the context of plant breeding programs, when choosing parents with outstanding traits to obtain progenies tolerant to salt stress.

Graphical Abstract

1. Introduction

Among the abiotic factors that affect the productivity of fruit orchards, the excess of salts at the rhizosphere is recognized as one of the more detrimental ones. The soil salinization is given majorly by natural factors but also by anthropic factors derived from some agricultural procedures, such as inappropriate practices of irrigation or overuse of fertilizers. These factors contribute to a continuous salinization process, which is a growing menace that currently is affecting around 20% of irrigated lands [1] and estimations foresee an increment close to 50% by the middle of this century [2]. Saline soils are defined as those with an electrical conductivity of the saturation extract (ECe) equal to or exceeding 4 dS/m [3]. This value determines significant reductions in the yield of the main crops worldwide [4].
In glycophyte plants, which include most crops, the impact of high salinity on plant growth is well known. Such a negative impact occurs in both the acute and chronic phases of salt stress. In first place, there is a reduction in the root water uptake ability as a consequence of the fall in the osmotic potential of the saline soil. The consequent osmotic stress triggers a reduction in cell expansion affecting root growth and leaf expansion alongside a drop in the stomatal conductance and photosynthesis rate [5]. In second place, the chronic accumulation of ions in plant tissues, such as sodium, imposes an ionic stress to the plant. At the leaf level, this ion toxicity could affect the enzyme activities, the production of photoassimilates, and, ultimately, the plant growth [6,7,8].
In general terms, the Prunus species are crops classified as sensitive to salinity within a range from moderate to highly salt sensitive [9], which implies the existence of a gradient of tolerance within the genetic background of this genus. Greater genetic diversity included in cultivated germplasm is pivotal for sustained crop improvement [10]. The characterization of this genetic diversity and its interaction with environmental factors are crucial for its adequate incorporation into plant breeding programs. The development of new stone fruit varieties with lower chilling requirements [11,12] has allowed to establish orchards in climatic zones with earlier harvesting seasons, such as semiarid regions [13] but with soils prone to saline conditions impairing the fruit production. In this context, the identification of germplasm with a higher ability to tolerate saline soils is particularly important to make viable the agriculture in such soil conditions and to perform studies aiming to reach a deeper insight into the mechanisms underlying their salt tolerance in woody fruit trees. Regarding the above mentioned, the development of rootstocks more tolerant to environmental challenges imposed by global climate change is key to adapting the modern fruit orchard production to adverse scenarios such as an excess or deficit of water, alkaline soils, and high salinity [14,15,16,17].
The root is the first organ to deal with the salt excess in soil, and given its functions of prospecting and transporting water, nutrients, and ions, it can play a key role in determining the sensitivity or tolerance to salt stress of the whole plant. In woody fruit trees with different levels of salt tolerance, a reduction in root growth under salt stress has been indistinctly evidenced [18,19,20,21]. Saline stress can imbalance the metabolism of reactive oxygen species (ROS) [22,23] and favor the accumulation of these molecules with deleterious effects at multiple levels such as DNA, lipids, proteins, photosynthetic pigments, cell membrane, among others [24,25,26]. In addition, the oxidative damage induced by excessive ROS accumulation has been involved as part of the decline of root growth in plants under saline stress [27,28]. Along with the detrimental effects on root growth, a reduction in root respiration has been reported as a high salinity effect [29]. Root respiration provides the energy necessary for both root growth and nutrient absorption [30], therefore, the inhibition of this process would imply a series of detrimental effects for physiological functions at the whole plant level [29]. At the aerial part of the plant, one of the consequences more widely reported of the salt stress is the negative impact on the photosynthetic rate (Pn), which in an early stage of the stress is given by stomatal limitations [31,32] and, latterly, by nonstomatal limitations [33].
Several studies covering different genotypes of the Prunus spp. have evidenced the impacts of the excess of salt on growth, biochemical and photosynthetic parameters, among others in order to characterize the ability of these woody species to adapt to salinity [21,34,35,36,37,38,39,40]. Although these studies have found different levels of tolerance to salt stress within the genus Prunus, it is important to consider that they usually include a small number of genotypes and that both the salinity levels and the methodologies for the imposition of saline stress differ between the investigations, which makes it difficult to estimate comparatively the ability to tolerate saline conditions and establish a well-defined gradient of salt tolerance among the Prunus species.
In this article, we characterize the responses of seven Prunus rootstock genotypes to salt stress imposed by watering with NaCl solutions ranging from 0 to 120 mM. These genotypes have different genetic backgrounds which aimed to perform a systematic study of the plant response to salt stress in the Prunus rootstocks germplasm in terms of root development, root respiration, oxidative damage, gas exchange, and water use efficiency. The salt tolerance coefficients of these genotypes were used to classify them according to their relative tolerance to high salinity (120 mM NaCl). This is a study that performed a systematic assessment of salt tolerance on the genotypes of rootstocks with a widely diverse genetic background that included species from the three subgenera of the Prunus genus and their hybrids. Such an evaluation is crucial to guide both the establishment of orchards with suitable rootstocks and the efforts of breeding programs for improving the ability of the Prunus rootstocks to better adapt to saline soils in order to sustain fruit production.

2. Material and Methods

2.1. Plant Material and Salt Stress Treatment

One-year-old, clonally propagated, and virus-free plants of the Prunus rootstock of ‘Mariana 2624’ (Prunus cerasifera × Prunus munsoniana W. Wight & Hedrick), ‘Cab 6P’ (Prunus cerasus L.), ‘Colt’ (Prunus avium (L.) L. × Prunus pseudocerasus Lindl.), ‘Maxma60’ (Prunus mahaleb L. × Prunus avium), ‘Garnem’ (G × N15) (Prunus dulcis (Mill.) D.A. Webb × (Prunus persica (L.) Batsch × Prunus davidiana (Carrière) N.E.Br.)), ‘Agaf 0204-09’ (Prunus persica × (Prunus dulcis × Prunus persica)), and ‘Mazzard F12/1’ (Prunus avium) genotypes were acquired from a commercial nursery and immediately transplanted to 3 L plastic pots. A mixture of sand, vermiculite, and perlite in a 1:1:1 ratio (v/v/v) was used as a substrate. Plants were watered three times a week with 200 mL of tap water and fertilized every two weeks with 1 g/pot of commercial fertilizer containing N:P:K (25:10:10) (UltrasolTM, Soquimich, Chile). Plants were grown in the CEAF’s (Centro de Estudios Avanzados en Fruticultura) experimental field (latitude 34°19’21.02″ S; longitude 70°50’02.26″ W) under semi controlled conditions under a plastic net where the PAR on the top of the plants was 700 mol m−2 s−1, and the temperature fluctuated between 27 and 30 °C in the day and 15 and 18 °C at night. The photoperiod during the experiment averaged 16/8 h day/night.
For salt stress treatment, sets of three plants of each genotype of the Prunus rootstocks were submitted to three salinity levels by watering with 0, 60 and 120 mM NaCl solutions with 0.83, 5.50 and 6.43 dS/m, respectively. These electrical conductivity values were recorded by an ExStick EC500 conductivimeter (Extech Instruments, Waltham, MA, USA). Plants were placed in greenhouse within controlled temperature ranging from 22 to 26 °C and watered regularly each third day with 400 mL of each solution for four weeks.

2.2. Root Length Measurement

At the end of the leaf gas exchange measurements, the plants were harvested, and their roots were carefully cleaned with water and shaken gently to remove excess water. Immediately, the roots were deployed on a smooth surface to be extended in order to record the maximum root length of their root systems. The maximum root length was determined as the length of the longest roots in each plant of the different genotypes under saline and control conditions. Finally, root samples were obtained for respiration rate and malondialdehyde content measurements.

2.3. Root Respiration Rate

Three rootstocks of each genotype submitted to three salinity levels were taken for root respiration measurements at the end of the experiment. To estimate root respiration rate (RRR), two sets of 2 cm segments of 10 root tips were excised from whole root system of each biological replicate. The root tips were enclosed and transferred in the dark to a root respiration airtight cuvette containing 3 mL of an oxygen-saturated nutrient solution without Fe to avoid element precipitation. The root respiration rate was measured as the O2 consumption from the root tips using a liquid-phase O2 electrode Clark-type (Hansatech Co. Ltd., Norlfolk, UK) connected to a constant temperature circulating water bath (Labtech, Singapore) at 25 °C. For each measurement point, the dissolved O2 concentration into the cuvette was continuously monitored and recorded every 5 min for 20 min. The nutrient solution into the root respiration cuvette was continuously homogenized with a magnetic stir bar at the bottom of the pots.

2.4. Malondialdehyde Determination

For the malondialdehyde (MDA) measurements, frozen roots (0.2 g) of each biological replicate were homogenized in 80% cold ethanol using a cold mortar and pestle. The homogenates were centrifuged, and two aliquots (technical replicates) of the supernatants were mixed with either 20% trichloroacetic acid or 20% trichloroacetic acid plus 0.5% thiobarbituric acid. Both mixtures were incubated at 90 °C for 1 h, cooled on ice and centrifuged at 3000× g for 10 min. The absorbance of each supernatant was measured at 440, 534, and 600 nm, and the MDA concentration was calculated according to [41].

2.5. Leaf Gas Exchange Measurements

The leaf gas exchange was measured according to [42], using a CIRAS-2 portable IRGA photosynthesis system (PPSystem, Hitchin, UK) with a controlled environment CIRAS PLC cuvette (broad windows 2.5 cm2) warmed at 25 °C. The incident PAR (1000 mmol m2 s1) was supplied by a LED light cuvette unit. The CO2 concentration in the cuvette was adjusted to 400 ppm, and the relative humidity was set at 50%. The stomatal conductance (gs), photosynthetic rate (A), transpiration rate (E), and internal CO2 concentration (Ci) were measured from 10:00 to 11:30 am on clear days on two fully expanded leaves from three plants of each genotype in the three experimental conditions at 0, 10, 20, and 30 days. The intrinsic water use efficiency (WUEi) was estimated from the ratio between the photosynthetic rate and stomatal conductance (A/gs).

2.6. Statistical Analysis

A randomized block design was used in the experiment. The means of two technical replicates of three independent biological replicates were subjected to one-way ANOVA and LSD pairwise comparisons using Statistica 4.0 software (Statsoft Inc., Tulsa, OK, USA).
Agglomerative hierarchical clustering was generated using salt tolerance coefficients (STCs). The STCs were calculated for growth, physiological, and biochemical parameters from their mean values registered at 30 days of treatment. STC = x̄salt/x̄control, where x̄salt is the mean value of the parameter under saline conditions, and x̄control is the mean value of the parameter under saline conditions. Dissimilarities among genotypes were established by the Euclidean distance and aggregated by Ward’s minimum variance method.

3. Results

3.1. Root Phenotype in Prunus spp. Rootstocks under Salt Stress

Different root phenotypes were observed among the seven Prunus rootstocks genotypes after 30 days of salt stress (Figure 1). As expected, the degree of root damage was related to the salinity level of the irrigation applied during this study.
At the end of the assay, among plants under the control condition (0 mM NaCl), two rootstock genotypes (‘Agaf 0204-09’ and ‘Maxma60’) presented the longest root systems with 27 cm approximately. The rest of the rootstocks exhibited similar root sizes ranging from 23.4 to 19.1 cm (Table 1).
In general terms, all genotypes of the Prunus rootstocks reduced the length of their root systems when exposed to 60 mM NaCl irrigation, but such reductions were more evident in plants treated with the 120 mM NaCl solution. In this saline concentration, the greatest reduction in the root length was recorded by the ‘Mazzard F12/1’ rootstock, decreasing to 55.67% with respect to the length measured in the control condition (Table 1). Interestingly, the two rootstock genotypes with the longest root systems registered in control conditions, exhibited opposite trends in salt stress. With NaCl 120 mM, ‘Agaf 0204-09’ was the rootstock with the least reduction of its root system size (20.35%). On the other hand, ‘Maxma60’ registered the second greatest reduction (48.44%) (Table 1).
Because the saline treatment with 120 mM NaCl revealed the largest impacts on the lengths of the root systems and established more clearly the differences in the tolerance/sensitivity degree among all the rootstock genotypes of the Prunus spp. in comparison to the root lengths under control conditions, the present study was focused on this saline stress level.

3.2. Malondialdehyde (MDA) Content in Roots

Along with the reduction of the root system length, salt-induced damage was also evidenced as a reddish coloration likely associated with the oxidation of the root tissue, which was more marked in roots under 120 mM NaCl irrigation at 30 days. In order to quantify the extension of this symptom, the MDA content was used as a biochemical marker of oxidative damage. In control conditions, the roots exhibited different MDA basal levels among the rootstocks analyzed, ranging from 0.88 nmol g−1 FW ± 0.37 (‘Colt’) to 2.15 nmol g−1 FW ± 0.28 (‘Mazzard F12/1’) (Figure 2). Expectedly, under salt stress, all genotypes showed a significant increase in their root MDA contents compared to those levels detected for the control plants. However, this increase in the MDA contents evidenced different magnitudes among the roots of the Prunus genotypes assessed. Thus, four out seven Prunus rootstocks did not double the amount of MDA produced in response to saline stress when compared to the levels detected in the control condition. In this group, ‘Mariana 2624’ roots evidenced the lowest MDA increment (54.58%) followed by ‘Garnem’ (63.24%), ‘Cab 6P’ (72.25%), and ‘Mazzard F12/1’ (81.44%). Instead, the other three rootstocks at least doubled their MDA contents, reaching the highest value in ‘Colt’ (154.64%), followed by ‘Maxma60’ (138.16%) and ‘Agaf 0204-09’ (107.02%) (Figure 2). Interestingly, the ‘Colt’ roots showed the highest percentage of increase in MDA contents despite being the genotype with the lowest basal levels of this marker of oxidative damage.

3.3. Root Respiration Rate

In control conditions, all the Prunus spp. rootstocks analyzed in this study showed similar RRRs, but when exposed to high salinity conditions (120 mM NaCl), this parameter was affected in a different extension depending on the genotype. Thus, the rootstocks evidencing the most marked drop in their RRRs were ‘Mazzard F12/1’ (78.62%) followed by ‘Garnem’ (78.26%, Figure 3). On the other hand, the ‘Mariana 2624’ roots exhibited the least decrease in RRR in saline conditions (52.97%, Figure 3) along with the lowest percentage of MDA concentration increase (Figure 2), however, this rootstock genotype suffered a noticeable reduction in its root length as a consequence of salt stress (Table 1).

3.4. Gas Exchange Parameters

The plants under control conditions showed stable values of photosynthetic rate (A) within genotypes in the measurements performed during the experiment (Figure 4A–G). As a consequence of salt stress, the photosynthetic rate was negatively affected in all rootstock genotypes (Figure 4H–N). However, the ‘Mazzard F12/1’rootstock exhibited the more rapid and dramatic drop since the assessment of the photosynthetic parameters evidenced an early A reduction of 68.73% (10 days of salinity), which was maintained until the end of the experiment (69.70% of A at 30 days) (Figure 4N). On the contrary, ‘Mariana 2624’ had the least fall in its values of photosynthetic rate in saline conditions showing reduced values in only 38.74% with respect to those detected in the control condition after 30 days of treatment (Figure 4H).
In a similar way as in the photosynthetic rate parameter, the stomatal conductance (gs) had similar values for the same genotype under control conditions throughout the experiment (Figure 5A–G). After 30 days of 120 mM NaCl irrigation, the largest reduction in gs values was evidenced in the ‘Maxma60’ genotype (88.30%, Figure 5K), followed by ‘Agaf 0204-09’ (85.79%, Figure 5J) and ‘Mazzard F12/1’ (81.79%, Figure 5N). Notably, the latter showed the strongest and most drastic stomatal closure, reaching its minimum values of gs as early as at 10 days of saline condition and maintaining them until the end of the assay (Figure 5N). In addition, ‘Mazzard F12/1’ evidenced the highest internal CO2 concentration (287.00 µL L−1) among all the salt stressed rootstocks (Suppl. Table S1).
On the other hand, ‘Garnem’ (67.55%, Figure 5L), ‘Mariana 2624’ (73.02%, Figure 5H), and ‘Colt’ (73.21%, Figure 5M) were the rootstock genotypes with the least reduction in gs. Interestingly, ‘Mariana 2624’ showed the highest value in this parameter (102.00 mmol H2O m−2 s−1) in comparison to the rest of the analyzed genotypes (Figure 5H–N). Beside this, ‘Mariana 2624’ was the rootstock genotype that evidenced the smaller drop in transpiration rate values (E, 51.95%) derived from saline irrigation at the end of the experiment (Suppl. Table S2).
The intrinsic water use efficiency (WUEi) was also calculated in order to further characterize the photosynthetic response of the Prunus spp. rootstocks to salt stress. Thus, the ‘Maxma 60’ and ‘Mariana 2624’ rootstocks reached the highest increments in WUEi values after 30 days of saline irrigation with 146.13% and 146.06% in comparison to the control values, respectively. The lower increment in WUEi values was recorded for ‘Mazzard F12/1’ with barely 63.63% (Figure 6).

3.5. Salt Tolerance Coefficients and Cluster Analysis

For each rootstock genotype, values from three parameters associated to root (maximum root length, root MDA, and root respiration rate) and six associated to leaf (leaf MDA, A, gs, Ci, E, and WUEi) were used to determine a ratio among their values recorded for plants under control and salt stressed conditions at the end of experiment after 30 days of treatments. These ratios denominated salt tolerance coefficients (STCs) were used as input for agglomerative hierarchical clustering. According to this analysis, the different Prunus spp. rootstocks were grouped into three major clusters: (I) ‘Mazzard F12/1’, (II) ‘Maxma 60’, ‘Cab6P’, and ‘AGAF 0204-09’; and (III) ‘Mariana 2624’, ‘Garnem’, and ‘Colt’ (Figure 7).

4. Discussion

Salt stress may cause a dramatic reduction in the productivity of different crops species present in arid and semiarid regions [43], but this problem is not restricted to those zones since it also affects some species, e.g., stone fruit trees grown in Mediterranean areas. In general terms, species of the Prunus genus are considered salt sensitive plants [9], however, it is feasible to detect some gradient of tolerance in commercial genotypes and wild relatives belonging to this genus [40]. Thus, in order to cope in adverse soil conditions that limit the development and production of these fruit trees, the use of rootstocks tolerant to biotic and/or abiotic factors turns out to be one of the best agronomic strategies to favor the establishment of orchards in such conditions [44,45].
In this study, we assessed the tolerance to long-term salt stress among seven Prunus genotypes used as rootstocks for cherries, plums, apricots, peaches, and almonds. The roots are the first plant organ in direct contact with excess salt and, despite that, they are considered more tolerant to salt stress compared to leaves; excess salt also triggers negative effects on the growth of the root system, such as reductions in biomass, elongation, and lateral development [46]. The root growth trait decreases in different magnitudes depending on the level of stress imposed and the intrinsic sensitivity of the genotypes at intra and interspecies levels. Usually, this trait can be expressed in terms of biomass or root length. Fruit trees with a degree of tolerance to salinity show a decrease in root biomass (dry weight) at NaCl concentrations as high as 200 and 300 mM as in the case of pomegranate (Punica granatum; L.) [47]. In Vitis vinifera accessions, the root relative growth rate (RGRr) fell between 36% and 40% under 150 mM NaCl [48]. In species very sensitive to salinity, e.g., avocado (Persea americana Mill.), the biomass (fresh weight) and root length decreases have been reported at low NaCl concentrations such as 9 mM [49] and 15 mM [18], respectively. Likewise, in olive (Olea europaea L.), a moderately salt tolerant plant, a more extensive reduction in the root biomass has been associated with more salt sensitive cultivars [19], and even the specific root length (SRL) fell from an electrical conductivity of 6 dS m−1 [50]. Moreover, in pistachio (Pistacia vera L.), a relatively salt tolerant fruit tree [51], a significative decrease of the root length at 150 mM NaCl has been reported [52]. Within fruit trees of the Prunus genus, the hybrid rootstock ‘GF667’ (P. amygdalus Batsch × P. persica (L.) evidenced a reduction in root growth parameters at NaCl concentrations ranging between 75 mM [37] and 120 mM [53]. The same was reported for the sour cherry rootstock ‘CAB 6P’ (Prunus cerasus L.) at 60 mM NaCl [21]. Moreover, an in vitro screening for the early detection of salt tolerance in Prunus spp. evidenced a reduction in the root length of rootstocks of the Cerasus (‘CAB 6P’ and ‘Masto de Montaña’) and Amygdalus (‘GF-667’) subgenera but not in those of the Prunus subgenus (‘Adesoto 101’ and ‘Mariana 2624’) [20]. In our work, we detected reductions of the root length in both saline levels but as expected, more markedly under 120 mM NaCl (Figure 1 and Table 1). Here, the hybrid ‘Agaf 0204-09’ (Amygdalus subgenus) was the rootstock with the least reduction in root length. On the other hand, ‘Mazzard F12/1’ turned out to be the genotype with the largest reduction in root length, which belongs to the subgenus Cerasus, this being the most affected in this trait as reported in the in vitro screening of [20].
As with other abiotic stresses, salt excess increases the production of reactive oxygen species (ROS), which triggers oxidative damage with detrimental impacts for plant tissue integrity [54]. The malondialdehyde (MDA), a lipoperoxidation product of disintegrated cell membranes, has been assessed as a biochemical marker of oxidative damage in roots by salt stress [55]. In maize (Zea mays L.), salinity-induced high MDA levels and oxidative stress affected more markedly the root tissues than the leaves [23]. However, an increase in MDA levels in the Prunus roots is not strictly coincident with a reduction in root length recorded in the rootstocks analyzed. For example, ‘Agaf 0204-09’, despite being the genotype with the lowest reduction in root length, is among the rootstocks that at least doubled their MDA levels in roots in response to saline stress (107.02% of increase relative to the control condition). On the other hand, ‘Mazzard F12/1’ showed a lower relative increase in MDA content (81.44%) but the greatest reduction in root length among genotypes. On the other hand, ‘Maxma 60’ showed a consistently negative impact on both root length and MDA levels detected in response to 120 mM NaCl.
Root respiration is sensitive to high levels of salinity in soils [56]. In the present study, all genotypes reduced root respiration under 120 mM NaCl, but a genotype-dependent variability was evidenced (Figure 3). According to [56], the respiratory rate responses under salinity conditions in plant tissues are complex, with 37% of studies reporting increases, 34% reporting decreases, and 29% reporting no consistent change in respiratory rate. In barley (Hordeum vulgare L.) cultivars with contrasting adaptive response to salinity, similar levels of root respiration were reported in the control condition. However, those genotypes showed an opposite behavior in their root respiration under salt stress (10 mM NaCl or KCl). The salt sensitive cultivar doubled its values of this parameter, but the salt tolerant one barely increased its root respiration to 50% and, additionally, showed a faster recovery after removal of the salt excess [57]. Conversely, in oak seedlings under high salinity (250 mM NaCl), root respiration was strongly inhibited, which was related to the arrest of root growth [58]. On the other hand, the halophyte species may increase root respiration in saline environments [59]. Root respiration is the major sink for carbohydrates [60], and it is separated into two principal components, “maintenance respiration” involved in the conservation of already existing tissue and “growth respiration” of new tissue [56]. In general, maintenance root respiration is key to providing energy and coping with stressful conditions, such as salinity [43,56]. The biomass accumulation in normal growth conditions represents between 10–40% of the total photosynthesis, while the maintenance mechanism represents the major investment [56]. Under saline conditions, root respiration has been observed to be increased but related principally with maintenance processes more than growth [43]. The elevated percentage of root respiration has been observed as dedicated to maintenance in plants under salt stress, principally associated to a significant demand of ATP provision to maintain transport processes against concentration gradient [61]. Thus, the Prunus spp. rootstock genotypes showed a variability in the impact of salt stress imposition on the components of their root respiration. A higher percentage of root respiration decrease was observed in ‘Garnem’, ‘Mazzard F12/1’, ‘Colt’, and ‘Agaf 0204-09’ than in ‘Cab 6P’, ‘Maxma 60’, and ‘Mariana 2624’ (Figure 3). Salinity showed the most detrimental effect on this parameter in the ‘Mazzard F12/1’ rootstock, whose roots also evidenced the largest decrease in root length (Table 1) and, additionally, the highest MDA concentration (Figure 2). Conversely, as happened with the MDA levels, ‘Mariana 2624’ showed the best response since it was the genotype that suffered the least reduction in the respiration of its roots, which possibly allowed for sufficient input energy to maintain its tissues and processes at the root level that are decisive in adaptation to saline stress.
The gas exchange is not only affected at the root level in plants under high salinity concentrations [61,62,63]. According to [43], the stress onset occurs when the amount of energy acquired by plants is reduced as a consequence of decreased A. In Prunus salicina, an experiment of long-term salt stress showed a complete inhibition of A under 28mM salt (mix NaCl and CaCl2) [64] and serious damage has been observed in the photosynthetic apparatus in the sweet almond [36], which may be an effect of fast stomatal closure as was observed in the grafted Prunus [53]. In our experiment, salinity stress (120 mM NaCl) reduced the A of all Prunus genotypes (Figure 4), ‘Mariana 2624’ being the rootstock with the least drop in this parameter and ‘Mazzard F12/1’ being the most affected. The reduction in photosynthesis was coupled with a drastic reduction in the gs (Figure 5). This may be associated with a CO2 limitation more than a biochemical one because a gs reduction may restrict the gas exchange as was observed in cotton plants by [65] and reviewed by [56]. Whereas here at the end of the saline stress treatment ‘Maxma60’ showed the greatest reduction in gs, the genotype that closed its stomata earlier was ‘Mazzard F12/1’. The fast reduction of gs under salt stress has been reported in previous studies [53,63,66] and showed that it could be beneficial to improve the WUEi. The WUEi reflects the balance between production (kg of biomass produced or moles of CO2 assimilated) and water costs (m3 of water used or moles of water transpired) by each plant and is commonly used to characterize the genetic effect and variability on a certain stress condition [67]. A comparative study including four wild Prunus species (Prunus maritima Marshall, P. salicina Lindl., P. cerasifera Ehrh., and P. persica (L.) Batsch) evidenced a consistent decrease in their gas exchange parameters in all genotypes after irrigation with a 100 mM NaCl solution although water use efficiency increased in the beach plum (P. maritima Marshall), a species that inhabits sandy coastal soils and is considered highly tolerant to salinity and drought [40]. Our results showed that WUEi increased in all the Prunus rootstock genotypes at the end of the salt stress experiment (Figure 6) but with variability among them. Thus, ‘Mariana 2624’ showed the highest increase in WUEi values in saline stress along with ‘Maxma 60’. On the contrary, ‘Mazzard F12/1’ showed the smallest increase in this parameter. The increasing WUEi observed is principally explained by the reduction in the gs (Figure 5) with respect to the A (Figure 4) as was observed in different studies [53,63,66]. A high WUEi indicates a better performance of the photosynthetic apparatus despite the stomatal closure triggered by the stress condition. In addition, a high WUEi may reduce the uptake of salt and alleviate the water deficiency induced by salinity [62] and thereby may be used as a good indicator of salt tolerance [63].
From the results obtained in this characterization of the adaptive response to salinity stress in rootstocks of the Prunus spp., both at the root and leaf levels, the ‘Mazzard F12/1’ rootstocks showed to be the genotype most negatively affected in most of the parameters evaluated. However, the best indices expected to be registered in a salinity tolerant genotype were not always indisputably associated with a single genotype. For instance, even though ‘Mariana 2624’ showed the best performances in several of the measurements, it also exhibited a significant reduction in root length under the 120 mM NaCl treatment. On the other hand, ‘Agaf 0204-09’ was the rootstock that showed the least reduction in root length, which could be clear evidence of a better tolerance of excess salt at the level of the root tissue present in this genotype, but it does not register the best values in other parameters in both root and leaf levels. In addition, the greatest increase in the WUEi value was detected in ‘Maxma 60’. As mentioned above, this parameter has been proposed as a good physiological index to characterize tolerance to stresses, such as drought and salinity, therefore, it would be expected that this rootstock would be among the Prunus genotypes most tolerant to saline stress. However, it was the second genotype with the greatest reduction in root length and accumulation of MDA under the 120 mM NaCl treatment. However, it was the second genotype with the greatest reduction in root length and accumulation of MDA under the 120 mM NaCl treatment. Given this complex scenario, an agglomerative clustering analysis was applied in order to group together data points according to their similarities and thus be able to discriminate the degree of tolerance to salt stress among the rootstocks analyzed. This type of analysis has been successfully used to characterize genotypes or accessions based on traits of interest in plant breeding programs [68,69,70].
In our analysis, the Prunus spp. rootstocks were grouped into three major clusters which were named considering the performance of the plant’s response to salt stress evidenced by the genotypes of each group. In this way, the most contrasting phenotypes in their response to saline stress (120 mM NaCl) were easily identifiable as ‘Mazzard F12/1’ (Prunus avium (L.) L.) (cluster I) being a very salt sensitive rootstock and ‘Mariana 2624’ (cluster III) being a salt tolerant rootstock. Although it shares cluster III with ‘Garnem’ and ‘Colt’, it is important to mention that ‘Mariana 2624’, a plum-based rootstock, showed better values in its parameters under stress conditions than its groupmates. This finding is consistent with previous reports that have indicated plum trees, members of the Prunus subgenus, as the species with the highest tolerance to salinity within the genus Prunus [9,35,40]. However, it is important to note that ‘Garnem’ (Prunus dulcis (Mill.) D.A. Webb × (Prunus persica (L.) Batsch × Prunus davidiana (Carrière) N.E.Br.)) and ‘Colt’ (Prunus avium (L.) L. × Prunus pseudocerasus Lindl.), as members of cluster III, represent excellent alternatives of salt tolerant rootstocks for productive varieties of the subgenera Amygdalus and Cerasus, respectively. In a classification of moderately tolerance to salt stress, cluster II mainly grouped rootstocks belonging to the Cerasus subgenus, i.e., ‘Cab 6P’ (Prunus cerasus L.) and ‘Maxma60’ (Prunus mahaleb L. × Prunus avium). These genotypes differ from the very salt sensitive genotype ‘Mazzard F12/1’, a cherry-based rootstock, for having a different or hybridized genetic background instead of only P. avium.

5. Conclusions

In the present work, an effective categorization of the adaptive response to salt stress of Prunus rootstocks was achieved from physiological measurements developed both at the root and leaf levels. An important aspect of this study is the inclusion of rootstocks (species and hybrids) whose genetic background covered the three subgenera (Prunus, Cerasus, and Amygdalus) with species of productive importance of the genus Prunus. The application of a multivariate analysis of agglomerative hierarchical clustering identified three clusters where the rootstocks were grouped based on their similarities in the behavior of their values in the physiological parameters analyzed. A tolerance gradient was established where the most contrasting genotypes in their tolerance to salt stress (120 mM NaCl) were ‘Mazzard F12/1’ (Prunus avium (L.) L.; subgenus Cerasus) and ‘Mariana 2624’ (Prunus cerasifera × Prunus munsoniana W. Wight & Hedrick; subgenus Prunus), being the most salt sensitive and the most salt tolerant, respectively.
An effective categorization of the adaptive response of plants is of crucial interest for the selection of parents with characteristics of interest in the framework of plant breeding programs. Moreover, it is valuable information when recommending rootstock alternatives to establish orchards in soils with edaphic problems, e.g., salinity due to a possible expansion of stone fruit orchards to new cultivation areas (arid or semiarid) due to the development of new productive varieties with lower chilling requirements.

Supplementary Materials

The following are available online at https://www.mdpi.com/article/10.3390/horticulturae7120542/s1. Table S1: Internal CO2 concentration (Ci) of Prunus rootstocks under control and 120 mM NaCl salt stress treatments. Table S2: Transpiration (E) of Prunus rootstocks under control and 120 mM NaCl salt stress treatments.

Author Contributions

Conceptualization, A.S. and G.T.; methodology, A.S. and G.T.; validation, A.S. and G.T.; formal analysis, A.S. and G.T.; investigation, A.S. and G.T.; resources, P.P.; data curation, A.S. and G.T.; original draft preparation, A.S.; review and editing, A.S., G.T. and. P.P.; visualization, A.S.; supervision, A.S. and G.T.; project administration, A.S.; funding acquisition, A.S. and P.P. All authors have read and agreed to the published version of the manuscript.

Funding

This work was funded by grants from Fondo Nacional de Desarrollo Científico y Tecnológico FONDECYT 11150393 and 1190816 and Agencia Nacional de Investigación y Desarrollo.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

Data are presented within the article and are available on request from the corresponding author.

Conflicts of Interest

The authors declare no conflict of interest.

References

  1. FAO. FAO Land and Plant Nutrition Management Service. 2008. Available online: http://www.fao.org/ag/agl/agll/spush (accessed on 5 February 2021).
  2. Jamil, A.; Riaz, S.; Ashraf, M.; Foolad, M.R. Gene expression profiling of plants under salt stress. Crit. Rev. Plant Sci. 2011, 30, 435–458. [Google Scholar] [CrossRef]
  3. Brown, G.E., Jr. Research Databases. Bibliography on Salt Tolerance. USDA-ARS US Dep. Agric. Res. Serv. Riverside CA 2008. Available online: https://www.ars.usda.gov/pacific-west-area/riverside-ca/agricultural-water-efficiency-and-salinity-research-unit/docs/research-databases/ (accessed on 21 December 2020).
  4. Munns, R. Genes and salt tolerance: Bringing them together. New Phytol. 2005, 167, 645–663. [Google Scholar] [CrossRef]
  5. Munns, R. Physiological processes limiting plant growth in saline soils: Some dogmas and hypotheses. stress. Plant Cell Environ. 1993, 16, 15–24. [Google Scholar] [CrossRef]
  6. Yu, J.; Chen, S.; Zhao, Q.; Wang, T.; Yang, C.; Diaz, C.; Sun, G.; Dai, S. Physiological and proteomic analysis of salinity tolerance in Puccinellia tenuiflora. J. Proteome Res. 2011, 10, 3852–3870. [Google Scholar] [CrossRef] [PubMed]
  7. Shu, S.; Guo, S.R.; Sun, J.; Yuan, L.Y. Effects of salt stress on the structure and function of the photosynthetic apparatus in Cucumis sativus and its protection by exogenous putrescine. Physiol. Plant. 2012, 146, 285–296. [Google Scholar] [CrossRef]
  8. Ashraf, M.; Harris, P.J.C. Photosynthesis under stressful environments: An overview. Photosynthetica 2013, 51, 163–190. [Google Scholar] [CrossRef]
  9. Kotuby-Amacher, J.; Koenig, R.; Kitchen, B. Salinity and Plant Tolerance; Utah State University Extension: Logan, UT, USA, 2000; AG-SO-03; Available online: https://digitalcommons.usu.edu/cgi/viewcontent.cgi?article=1042&context=extension_histall (accessed on 12 December 2020).
  10. Byrne, P.F.; Volk, G.M.; Gardner, C.; Gore, M.A.; Simon, P.W.; Smith, S. Sustaining the future of plant breeding: The critical role of the USDA-ARS National Plant Germplasm System. Crop Sci. 2018, 58, 451–468. [Google Scholar] [CrossRef] [Green Version]
  11. Sansavini, S.; Lugli, S. Sweet cherry breeding programs in Europe and Asia. Acta Hortic. 2008, 795, 41–58. [Google Scholar] [CrossRef] [Green Version]
  12. Sawamura, Y.; Suesada, Y.; Sugiura, T.; Yaegaki, H. Chilling requirements and blooming dates of leading peach cultivars and a promising early maturing peach selection, Momo Tsukuba 127. Hortic. J. 2017, 86, 426–436. [Google Scholar] [CrossRef] [Green Version]
  13. Apey, A. La Fruticultura en Chile: Tendencias Productivas y su Expresión Territorial. 2019. Available online: https://www.odepa.gob.cl/publicaciones/articulos/la-fruticultura-en-chile-tendencias-productivas-y-su-expresion-territorial (accessed on 26 February 2021).
  14. Ikinci, A.; Bolat, I.; Ercisli, S.; Kodad, O. Influence of rootstocks on growth, yield, fruit quality and leaf mineral element contents of pear cv. ‘Santa Maria’ in semi-arid conditions. Biol. Res. 2014, 47, 1–8. [Google Scholar] [CrossRef] [Green Version]
  15. Marguerit, E.; Brendel, O.; Lebon, E.; van Leeuwen, C.; Ollat, N. Rootstock control of scion transpiration and its acclimation to water deficit are controlled by different genes. New Phytol. 2012, 194, 416–429. [Google Scholar] [CrossRef] [PubMed]
  16. Peccoux, A.; Loveys, B.; Zhu, J.; Gambetta, G.A.; Delrot, S.; Vivin, P.; Schultz, H.R.; Ollat, N.; Dai, Z. Dissecting the rootstock control of scion transpiration using model-assisted analyses in grapevine. Tree Physiol. 2018, 38, 1026–1040. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  17. Tamura, F. Recent advances in research on Japanese pear rootstocks. J. Jpn. Soc. Hortic. Sci. 2012, 81, 1–10. [Google Scholar] [CrossRef]
  18. Bernstein, N.; Meiri, A.; Zilberstaine, M. Root growth of avocado is more sensitive to salinity than shoot growth. J. Am. Soc. Hortic. Sci. 2004, 129, 188–192. [Google Scholar] [CrossRef]
  19. Rewald, B.; Leuschner, C.; Wiesman, Z.; Ephrath, J.E. Influence of salinity on root hydraulic properties of three olive varieties. Plant Biosyst. 2011, 145, 12–22. [Google Scholar] [CrossRef]
  20. Andreu, P.; Arbeloa, A.; Lorente, P.; Marín, J.A. Early detection of salt stress tolerance of Prunus rootstocks by excised root culture. HortScience 2011, 46, 80–85. [Google Scholar] [CrossRef]
  21. Papadakis, I.E.; Veneti, G.; Chatzissavvidis, C.; Therios, I. Physiological and growth responses of sour cherry (Prunus cerasus L.) plants subjected to short-term salinity stress. Acta Bot. Croat. 2018, 77, 197–202. [Google Scholar] [CrossRef] [Green Version]
  22. Tanou, G.; Molassiotis, A.; Diamantidis, G. Hydrogen peroxide-and nitric oxide-induced systemic antioxidant prime-like activity under NaCl-stress and stress-free conditions in citrus plants. J. Plant Physiol. 2009, 166, 1904–1913. [Google Scholar] [CrossRef] [PubMed]
  23. AbdElgawad, H.; Zinta, G.; Hegab, M.; Pandey, R.; Asard, H.; Abuelsoud, W. High salinity induces different oxidative stress and antioxidant responses in maize seedlings organs. Front. Plant Sci. 2016, 7, 276. [Google Scholar] [CrossRef] [Green Version]
  24. Imlay, J.A.; Linn, S. DNA damage and oxygen radical toxicity. Science 1988, 240, 1302–1309. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  25. Noctor, G.; Foyer, C.H. Ascorbate and glutathione: Keeping active oxygen under control. Annu. Rev. Plant Physiol. Plant Mol. Biol. 1998, 49, 249–279. [Google Scholar] [CrossRef] [PubMed]
  26. Pitzschke, A.; Forzani, C.C.; Hirt, H. Reactive oxygen species signaling in plants. Antiox. Redox Signal. 2006, 8, 1757–1764. [Google Scholar] [CrossRef]
  27. Katsuhara, M.; Otsuka, T.; Ezaki, B. Salt stress-induced lipid peroxidation is reduced by glutathione S-transferase, but this reduction of lipid peroxides is not enough for a recovery of root growth in Arabidopsis. Plant Sci. 2005, 69, 369–373. [Google Scholar] [CrossRef]
  28. Maia, J.M.; Voigt, E.L.; Macêdo, C.E.C.; Ferreira-Silva, S.L.; Silveira, J.A.G. Salt-induced changes in antioxidative enzyme activities in root tissues do not account for the differential salt tolerance of two cowpea cultivars. Braz. J. Plant Physiol. 2010, 22, 113–122. [Google Scholar] [CrossRef] [Green Version]
  29. Khataar, M.; Mohammadi, M.; Shabani, F. Soil salinity and matric potential interaction on water use, water use efficiency and yield response factor of bean and wheat. Sci. Rep. 2018, 8, 2679. [Google Scholar] [CrossRef] [PubMed]
  30. Lambers, H. Respiration associated with growth, maintenance, and ion uptake. In Plant Physiological Ecology; Lambers, H., Chapin, F., Pons, T.L., Eds.; Springer: New York, NY, USA, 2008; pp. 134–140. [Google Scholar]
  31. Moya, J.L.; Primo-Millo, E.; Talon, M. Morphological factors determining salt tolerance in citrus seedlings: The shoot to root ratio modulates passive root uptake of chloride ions and their accumulation in leaves. Plant Cell Environ. 1999, 22, 1425–1433. [Google Scholar] [CrossRef]
  32. Rajendran, K.; Tester, M.; Roy, S.J. Quantifying the three maincomponents of salinity tolerance in cereals. Plant Cell Environ. 2009, 32, 237. [Google Scholar] [CrossRef] [PubMed]
  33. Chaves, M.M.; Flexas, J.; Pinheiro, C. Photosynthesis under drought and salt stress: Regulation mechanisms from whole plant to cell. Ann. Bot. 2009, 103, 551–560. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  34. El-Motaium, R.; Hu, H.; Brown, P.H. The relative tolerance of six Prunus rootstocks to boron and salinity. J. Am. Soc. Hortic. Sci. 1994, 119, 1169–1175. [Google Scholar] [CrossRef]
  35. Rieger, M. Salt stress resistance of peach and four north american Prunus species. Acta Hortic. 2001, 557, 181–192. [Google Scholar] [CrossRef]
  36. Ranjbarfordoei, A.; Samson, R.; Van Damme, P. Chlorophyll fluorescence performance of sweet almond (Prunus dulcis (Miller) D. Webb) in response to salinity stress induced by NaCl. Photosynthetica 2006, 44, 513–522. [Google Scholar] [CrossRef]
  37. Najafian, S.; Rahemi, M.; Tavallali, V. Effect of salinity on tolerance of two bitter almond rootstocks. Am.-Eurasian J. Agri. Environ. Sci. 2008, 3, 264–268. [Google Scholar]
  38. Küçükyumuk, C.; Yildiz, H.; Küçükyumuk, Z.; Ünlükara, A. Responses of ‘0900 Ziraat’ sweet cherry variety grafted on different rootstocks to salt stress. Not. Bot. Horti Agrobot. Cluj-Napoca 2015, 43, 214–221. [Google Scholar] [CrossRef] [Green Version]
  39. Zrig, A.; Mohamed, H.B.; Tounekti, T.; Ennajeh, M.; Valero, D.; Khemira, H. A comparative study of salt tolerance of three almond rootstocks: Contribution of organic and inorganic solutes to osmotic adjustment. J. Agr. Sci. Tech. 2015, 17, 675–689. [Google Scholar]
  40. Wang, X.M.; Huang, T.; Wu, W.L.; Li, W.L.; Zhu, H. Effects of salt stress on photosynthetic characteristics of beach plum and other Prunus species. Acta Hortic. 2016, 1112, 233–240. [Google Scholar]
  41. Arbona, V.; Hossain, Z.; Lopez-Climent, M.F.; Perez-Clemente, R.M.; Gomez-Cadenas, A. Antioxidant enzymatic activity is linked to waterlogging stress tolerance in citrus. Physiol. Plant. 2008, 132, 452–466. [Google Scholar] [CrossRef] [PubMed]
  42. Pimentel, P.; Almada, R.D.; Salvatierra, A.; Toro, G.; Arismendi, M.J.; Pino, M.T.; Sagredo, B.; Pinto, M. Physiological and morphological responses of Prunus species with different degree of tolerance to long-term root hypoxia. Sci. Hortic. 2014, 180, 14–23. [Google Scholar] [CrossRef]
  43. Munns, R.; Gilliham, M. Salinity tolerance of crops–what is the cost? New Phytol. 2015, 208, 668–673. [Google Scholar] [CrossRef] [Green Version]
  44. Gainza, F.; Opazo, I.; Guajardo, V.; Meza, P.; Ortiz, M.; Pinochet, J.; Muñoz, C. Rootstock breeding in Prunus species: Ongoing efforts and new challenges. Chil. J. Agric. Res. 2015, 75, 6–16. [Google Scholar] [CrossRef] [Green Version]
  45. Nimbolkar, P.K.; Awachare, C.; Reddy, Y.T.N.; Chander, S.; Hussain, F. Role of rootstocks in fruit production–A Review. J. Agric. Eng. Food Technol. 2016, 3, 183–188. [Google Scholar]
  46. Shahzad, A.; Ahmad, M.; Iqbal, M.; Ahmed, I.; Ali, G. Evaluation of wheat landrace genotypes for salinity tolerance at vegetative stage by using morphological and molecular markers. Genet. Mol. Res. 2012, 11, 679–692. [Google Scholar] [CrossRef]
  47. Cuiyu, L.; Ming, Y.; Xianbin, H.; Zhaohe, Y. Effects of NaCl stress on growth and ion homeostasis in pomegranate tissues. Eur. J. Hortic. Sci. 2020, 85, 42–50. [Google Scholar] [CrossRef]
  48. Askri, H.; Daldoul, S.; Ammar, A.B.; Rejeb, S.; Jardak, R.; Rejeb, M.N.; Mliki, A.; Ghorbel, A. Short-term response of wild grapevines (Vitis vinifera L. ssp. sylvestris) to NaCl salinity exposure: Changes of some physiological and molecular characteristics. Acta Physiol. Plant. 2012, 34, 957–968. [Google Scholar] [CrossRef]
  49. Bonomelli, C.; Celis, V.; Lombardi, G.; Mártiz, J. Salt stress effects on avocado (Persea americana Mill.) plants with and without seaweed extract (Ascophyllum nodosum) application. Agronomy 2018, 8, 64. [Google Scholar] [CrossRef] [Green Version]
  50. Tan, J.; Ben-Gal, J.; Shtein, I.; Bustan, A.; Dag, A.; Erel, R. Root structural plasticity enhances salt tolerance in mature olives. Environ. Exp. Bot. 2020, 179, 104224. [Google Scholar] [CrossRef]
  51. Picchioni, G.A.; Miyamoto, S.; Storey, J.B. Salt effects on growth and ion uptake of pistachio rootstock seedlings. J. Am. Soc. Hortic. Sci. 1990, 115, 647–653. [Google Scholar] [CrossRef]
  52. Rahneshan, Z.; Nasibi, F.; Moghadam, A.H. Effects of salinity stress on some growth, physiological, biochemical parameters and nutrients in two pistachio (Pistacia vera L.) rootstocks. J. Plant Interact. 2018, 13, 73–82. [Google Scholar] [CrossRef] [Green Version]
  53. Massai, R.; Remorini, D.; Tattini, M. Gas exchange, water relations and osmotic adjustment in two scion/rootstock combinations of Prunus under various salinity concentrations. Plant Soil 2004, 259, 153–162. [Google Scholar] [CrossRef]
  54. Gill, S.S.; Tuteja, N. Reactive oxygen species and antioxidant machinery in abiotic stress tolerance in crop plants. Plant Physiol. Biochem. 2010, 48, 909–930. [Google Scholar] [CrossRef]
  55. Al Kharusi, L.; Al Yahyai, R.; Yaish, M.W. Antioxidant response to salinity in Salt-Tolerant and Salt-Susceptible cultivars of date palm. Agriculture 2019, 9, 8. [Google Scholar] [CrossRef] [Green Version]
  56. Jacoby, R.P.; Taylor, N.L.; Millar, A.H. The role of mitochondrial respiration in salinity tolerance. Trends Plant Sci. 2011, 16, 614–623. [Google Scholar] [CrossRef] [PubMed]
  57. Bloom, A.; Epstein, E. Varietal differences in salt-induced respiration in barley. Plant Sci. Lett. 1984, 35, 1–3. [Google Scholar] [CrossRef]
  58. Epron, D.; Toussaint, M.-L.; Badot, P.-M. Effects of sodium chloride salinity on root growth and respiration in oak seedlings. Ann. For. Sci. 1999, 56, 41–47. [Google Scholar] [CrossRef]
  59. Hwang, Y.-H.; Morris, J.T. Whole-plant gas exchange responses of Spartina alterniflora (Poaceae) to a range of constant and transient salinities. Am. J. Bot. 1994, 81, 659–665. [Google Scholar] [CrossRef]
  60. Rachmilevitch, S.; Lambers, H.; Huang, B. Root respiratory characteristics associated with plant adaptation to high soil temperature for geothermal and turf-type Agrostis species. J. Exp. Bot. 2006, 57, 623–631. [Google Scholar] [CrossRef] [Green Version]
  61. Schwarz, M.; Gale, J. Maintenance respiration and carbon balance of plants at low levels of sodium chloride salinity. J. Exp. Bot. 1981, 32, 933–5941. [Google Scholar] [CrossRef]
  62. Karaba, A.; Dixit, S.; Greco, R.; Aharoni, A.; Trijatmiko, K.R.; Marsch-Martinez, N.; Krishnan, A.; Nataraja, K.N.; Udayakumar, M.; Pereira, A. Improvement of water use efficiency in rice by expression of HARDY, an Arabidopsis drought and salt tolerance gene. Proc. Natl. Acad. Sci. USA 2007, 104, 15270–15275. [Google Scholar] [CrossRef] [Green Version]
  63. Omamt, E.N.; Hammes, P.S.; Robbertse, P.J. Differences in salinity tolerance for growth and water-use efficiency in some amaranth (Amaranthus spp.) genotypes. N. Z. J. Crop Hortic. Sci. 2006, 34, 11–22. [Google Scholar] [CrossRef]
  64. Ziska, L.H.; Seemann, J.R.; DeJong, T.M. Salinity induced limitations on photosynthesis in Prunus salicina, a deciduous tree species. Plant Physiol. 1990, 93, 864–870. [Google Scholar] [CrossRef] [Green Version]
  65. Meloni, D.A.; Oliva, M.A.; Martinez, C.A.; Cambraia, J. Photosynthesis and activity of superoxide dismutase, peroxidase and glutathione reductase in cotton under salt stress. Environ. Exp. Bot. 2003, 49, 69–76. [Google Scholar] [CrossRef]
  66. Rouphael, Y.; Cardarelli, M.; Rea, E.; Colla, G. Improving melon and cucumber photosynthetic activity, mineral composition, and growth performance under salinity stress by grafting onto Cucurbita hybrid rootstocks. Photosynthetica 2012, 50, 180–188. [Google Scholar] [CrossRef]
  67. Tomás, M.; Medrano, H.; Escalona, J.M.; Martorell, S.; Pou, A.; Ribas-Carbó, M.; Flexas, J. Variability of water use efficiency in grapevines. Environ. Exp. Bot. 2014, 103, 148–157. [Google Scholar] [CrossRef]
  68. Yin, R.; Bai, T.; Ma, F.; Wang, X.; Li, Y.; Yue, Z. Physiological responses and relative tolerance by Chinese apple rootstocks to NaCl stress. Sci. Hortic. 2010, 126, 247–252. [Google Scholar] [CrossRef]
  69. Ganopoulos, I.; Tourvas, N.; Xanthopoulou, A.; Aravanopoulos, F.A.; Avramidou, E.; Zambounis, A.; Tsaftaris, A.; Madesis, P.; Sotiropoulos, T.; Koutinas, N. Phenotypic and molecular characterization of apple (Malus × domestica Borkh) genetic resources in Greece. Sci. Agric. 2018, 75, 509–518. [Google Scholar] [CrossRef] [Green Version]
  70. Goharrizi, K.J.; Baghizadeh, A.; Kalantar, M.; Fatehi, F. Combined effects of salinity and drought on physiological and biochemical characteristics of pistachio rootstocks. Sci. Hortic. 2020, 261, 108970. [Google Scholar] [CrossRef]
Horticulturae 07 00542 g001 550
Figure 1. Representative phenotypes of the seven Prunus rootstock genotypes assayed after 30 days of saline treatment. Roots under control irrigation with distillated water: (A) ‘Mariana 2624’, (B) ‘Cab6P’, (C) ‘AGAF 0204-09’, (D) ‘Maxma 60’, (E) ‘Garnem’, (F) ‘Colt’, and (G) ‘Mazzard F12/1’. Roots under saline irrigation with 60 mM NaCl solution: (H) ‘Mariana 2624’, (I) ‘Cab6P’, (J) ‘AGAF 0204-09’, (K) ‘Maxma 60’, (L) ‘Garnem’, (M) ‘Colt’, and (N) ‘Mazzard F12/1’. Roots under saline irrigation with 120 mM NaCl solution: (O) ‘Mariana 2624’, (P) ‘Cab6P’, (Q) ‘AGAF 0204-09’, (R) ‘Maxma 60’, (S) ‘Garnem’, (T) ‘Colt’, and (U) ‘Mazzard F12/1’. Scale bar: 10 cm.
Figure 1. Representative phenotypes of the seven Prunus rootstock genotypes assayed after 30 days of saline treatment. Roots under control irrigation with distillated water: (A) ‘Mariana 2624’, (B) ‘Cab6P’, (C) ‘AGAF 0204-09’, (D) ‘Maxma 60’, (E) ‘Garnem’, (F) ‘Colt’, and (G) ‘Mazzard F12/1’. Roots under saline irrigation with 60 mM NaCl solution: (H) ‘Mariana 2624’, (I) ‘Cab6P’, (J) ‘AGAF 0204-09’, (K) ‘Maxma 60’, (L) ‘Garnem’, (M) ‘Colt’, and (N) ‘Mazzard F12/1’. Roots under saline irrigation with 120 mM NaCl solution: (O) ‘Mariana 2624’, (P) ‘Cab6P’, (Q) ‘AGAF 0204-09’, (R) ‘Maxma 60’, (S) ‘Garnem’, (T) ‘Colt’, and (U) ‘Mazzard F12/1’. Scale bar: 10 cm.
Horticulturae 07 00542 g001
Horticulturae 07 00542 g002 550
Figure 2. MDA concentrations in the roots of Prunus rootstocks under salt stress treatments. Levels under control condition (white bars) and 120 mM NaCl (gray bars) saline irrigation. The values and error bars represent the mean and standard errors of three biological replicates with two technical replicates. Different letters indicate significant (p < 0.05) differences among genotypes within the same treatment. Dots represent the percentage of increase in MDA levels between control and salt treatments for each rootstock genotype.
Figure 2. MDA concentrations in the roots of Prunus rootstocks under salt stress treatments. Levels under control condition (white bars) and 120 mM NaCl (gray bars) saline irrigation. The values and error bars represent the mean and standard errors of three biological replicates with two technical replicates. Different letters indicate significant (p < 0.05) differences among genotypes within the same treatment. Dots represent the percentage of increase in MDA levels between control and salt treatments for each rootstock genotype.
Horticulturae 07 00542 g002
Horticulturae 07 00542 g003 550
Figure 3. Root respiration rate of Prunus rootstocks under salt stress treatments. Levels under control condition (white bars) and 120 mM NaCl (gray bars) saline irrigation. The values and error bars represent the mean and standard errors of three biological replicates with two technical replicates. Different letters indicate significant (p < 0.05) differences among genotypes within the same treatment. Dots represent the percentage of decrease in root respiration levels between control and salt treatments for each rootstock genotype.
Figure 3. Root respiration rate of Prunus rootstocks under salt stress treatments. Levels under control condition (white bars) and 120 mM NaCl (gray bars) saline irrigation. The values and error bars represent the mean and standard errors of three biological replicates with two technical replicates. Different letters indicate significant (p < 0.05) differences among genotypes within the same treatment. Dots represent the percentage of decrease in root respiration levels between control and salt treatments for each rootstock genotype.
Horticulturae 07 00542 g003
Horticulturae 07 00542 g004 550
Figure 4. Photosynthetic rate (A) of Prunus rootstocks under control (AG) and 120 mM NaCl salt stress (HN) treatments. The values and error bars represent the mean and standard errors of four biological replicates with three technical replicates. Different letters indicate significant (p < 0.05) differences within a genotype during 30 days of treatments.
Figure 4. Photosynthetic rate (A) of Prunus rootstocks under control (AG) and 120 mM NaCl salt stress (HN) treatments. The values and error bars represent the mean and standard errors of four biological replicates with three technical replicates. Different letters indicate significant (p < 0.05) differences within a genotype during 30 days of treatments.
Horticulturae 07 00542 g004
Horticulturae 07 00542 g005 550
Figure 5. Stomatal conductance (gs) of Prunus rootstocks under control (AG) and 120 mM NaCl salt stress (HN) treatments. The values and error bars represent the mean and standard error of four biological replicates with three technical replicates. Different letters indicate significant (p < 0.05) differences within a genotype during 30 days of treatments.
Figure 5. Stomatal conductance (gs) of Prunus rootstocks under control (AG) and 120 mM NaCl salt stress (HN) treatments. The values and error bars represent the mean and standard error of four biological replicates with three technical replicates. Different letters indicate significant (p < 0.05) differences within a genotype during 30 days of treatments.
Horticulturae 07 00542 g005
Horticulturae 07 00542 g006 550
Figure 6. Intrinsic water use efficiency (WUEi) of Prunus rootstocks under control (AG) and 120 mM NaCl salt stress (HN) treatments. The values and error bars represent the mean and standard errors of four biological replicates with three technical replicates. Different letters indicate significant (p < 0.05) differences within a genotype during 30 days of treatments.
Figure 6. Intrinsic water use efficiency (WUEi) of Prunus rootstocks under control (AG) and 120 mM NaCl salt stress (HN) treatments. The values and error bars represent the mean and standard errors of four biological replicates with three technical replicates. Different letters indicate significant (p < 0.05) differences within a genotype during 30 days of treatments.
Horticulturae 07 00542 g006
Horticulturae 07 00542 g007 550
Figure 7. Dendrogram of the agglomerative hierarchical clustering of Prunus spp. rootstocks based on salt tolerance coefficients (STC). Dashed line indicates the dissimilarity threshold defining the number of rootstocks clusters within the analysis.
Figure 7. Dendrogram of the agglomerative hierarchical clustering of Prunus spp. rootstocks based on salt tolerance coefficients (STC). Dashed line indicates the dissimilarity threshold defining the number of rootstocks clusters within the analysis.
Horticulturae 07 00542 g007
Table
Table 1. Variations of the root system length of Prunus rootstocks under salt stress treatments.
Table 1. Variations of the root system length of Prunus rootstocks under salt stress treatments.
Maximum Root Length (cm)
NaCl Solution Concentration
0 mM60 mM120 mM
Mariana 262423.4 a±1.916.6 b±3.713.9 b±1.7
Cab 6P20.2 a±3.017.0 a±1.115.0 b±0.8
Agaf 0204-0927.4 a±1.823.0 b±1.321.9 b±1.3
Maxma6027.8 a±2.913.7 b±2.814.4 b±1.6
Garnem19.6 a±2.014.7 b±1.012.4 b±2.4
Colt21.0 a±1.617.0 b±0.815.1 c±0.4
Mazzard F12/119.1 a±1.813.9 b±1.88.5 c±2.1
The values represent the mean and standard error of three biological replicates. The different letters indicate significant (p < 0.05) differences among treatments within a genotype after 30 days of salt stress treatments.
Publisher’s Note: MDPI stays neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Share and Cite

MDPI and ACS Style

Toro, G.; Pimentel, P.; Salvatierra, A. Effective Categorization of Tolerance to Salt Stress through Clustering Prunus Rootstocks According to Their Physiological Performances. Horticulturae 2021, 7, 542. https://doi.org/10.3390/horticulturae7120542

AMA Style

Toro G, Pimentel P, Salvatierra A. Effective Categorization of Tolerance to Salt Stress through Clustering Prunus Rootstocks According to Their Physiological Performances. Horticulturae. 2021; 7(12):542. https://doi.org/10.3390/horticulturae7120542

Chicago/Turabian Style

Toro, Guillermo, Paula Pimentel, and Ariel Salvatierra. 2021. "Effective Categorization of Tolerance to Salt Stress through Clustering Prunus Rootstocks According to Their Physiological Performances" Horticulturae 7, no. 12: 542. https://doi.org/10.3390/horticulturae7120542

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop