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Article

Priming of Resistance-Related Phenolics: A Study of Plant-Associated Bacteria and Hymenoscyphus fraxineus

by
Greta Striganavičiūtė
,
Jonas Žiauka
,
Vaida Sirgedaitė-Šėžienė
* and
Dorotėja Vaitiekūnaitė
Laboratory of Forest Plant Biotechnology, Institute of Forestry, Lithuanian Research Centre for Agriculture and Forestry, Liepų Str. 1, Girionys, LT-53101 Kaunas, Lithuania
*
Author to whom correspondence should be addressed.
Microorganisms 2021, 9(12), 2504; https://0-doi-org.brum.beds.ac.uk/10.3390/microorganisms9122504
Submission received: 4 November 2021 / Revised: 29 November 2021 / Accepted: 1 December 2021 / Published: 2 December 2021
(This article belongs to the Special Issue Plant Associated Bacteria, so Different and so Similar: From Pathogens to Symbionts and to Biological Control Agents)
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Abstract

:
European ash (Fraxinus excelsior) is highly affected by the pathogenic fungus Hymenoscyphus fraxineus in all of Europe. Increases in plant’s secondary metabolite (SM) production is often linked tol enhanced resistance to stress, both biotic and abiotic. Moreover, plant-associated bacteria have been shown to enhance SM production in inoculated plants. Thus, our hypothesis is that bacteria may boost ash SM production, hence priming the tree’s metabolism and facilitating higher levels of resilience to H. fraxineus. We tested three different ash genotypes and used Paenibacillus sp. and Pseudomonas sp. for inoculation in vitro. Total phenol (TPC), total flavonoid (TFC) and carotenoid contents were measured, as well as the chlorophyll a/b ratio and morphometric growth parameters, in a two-stage trial, whereby seedlings were inoculated with the bacteria during the first stage and with H. fraxineus during the second stage. While the tested bacteria did not positively affect the morphometric growth parameters of ash seedlings, they had a statistically significant effect on TPC, TFC, the chlorophyll a/b ratio and carotenoid content in both stages, thus confirming our hypothesis. Specifically, in ash genotype 64, both bacteria elicited an increase in carotenoid content, TPC and TFC during both stages. Additionally, Pseudomonas sp. inoculated seedlings demonstrated an increase in phenolics after infection with the fungus in both genotypes 64 and 87. Our results indicate that next to genetic selection of the most resilient planting material for ash reforestation, plant-associated bacteria could also be used to boost ash SM production.

1. Introduction

Under modern climate change conditions, there is a massive weakening of trees due to the spread of pests and diseases in forests, which result in huge economic, genetic and biodiversity losses. Therefore, more attention should be paid to the increase in forest resistance and productivity as they are associated with the negative effects of pathogens, by selecting tree genotypes that are resistant to these disadvantageous factors [1,2,3,4].
European ash (Fraxinus excelsior L.) is a valuable hardwood species in forest ecosystems as well as in the open landscape. Furthermore, this tree species is important due to its economic value and related biodiversity [5,6,7]. Over the last 20 years, an epidemic of ash dieback (ADB), caused by the fungal pathogen Hymenoscyphus fraxineus (syn. Chalara fraxinea/H. pseudoalbidus), has spread throughout Europe and is drastically reducing European ash populations [8]. According to the data of the State Forest Service, European ash is a vulnerable tree species in Lithuanian forests. Data show that, in 2020, 13% of the total forest trees were damaged by diseases and 34.15% of them suffered from H. fraxineus [9]. This disease leads to widespread dieback and tree mortality, therefore, most concerningly, it may result in a substantial reduction or even loss of F. excelsior in most of Europe [8,10,11]. Thus, due to the rapid and widespread occurrence and intensification of this disease, the management of European ash has become increasingly challenging.
Research indicates that bacteria and fungi, which live in the plant episphere and endosphere, can directly decrease the negative impact of invaders through resource competition, parasitism and antibiosis, or, indirectly, by activating the plant’s defense system [12,13]. Moreover, some endophytic microorganisms are able to promote plant growth and development, resulting in an increased resilience in response to stress and pathogens [14,15]. These processes can be caused by microorganisms’ interaction with their host’s metabolism and environmental conditions [16,17]. Plant-growth-promoting bacteria are used as an eco-friendly alternative to chemical fertilizers and pesticides in agriculture [18,19]. However, studies of culturable bacteria and their antagonistic potential in forestry are still lacking [20,21].
Several studies have reported that 1–5% of European ash genotypes may possess a durable, high, but partial resistance to H. fraxineus [11,22,23,24,25,26,27]. Tree resistance to pathogens is related to their ability to synthesize and mobilize secondary metabolites (SMs) [2,28,29,30,31], since these SMs (ex. phenolics) may perform numerous protective functions and their amount is related to general or specific plant pathogenic resistance [2,28,32,33]. Some studies have reported that endophytic bacteria can affect plants’ secondary metabolism [30,34,35]. Moreover, recent studies have shown that plant-associated microorganisms can be antagonists to H. fraxineus and potentially serve as a tool for ash protection [21,36]. However, we have found no systematic studies related to the impact of different symbiotic bacteria on the formation of pathogenic resistance via SM production in F. excelsior as it relates to H. fraxineus infection. Additionally, studies show that different genotypes have different abilities to synthesize SM, therefore the genetic selection of resilient genotypes is appropriate [2,28,32,33].
Bacteria from Paenibacillus and Pseudomonas genera and their effect on trees have been studied in several works [37,38,39]. Bacteria from both genera have also been studied in relation to antimicrobial use [40,41,42], likely in part due to their potential for chitinase production [43,44]. Previously, we have shown that both bacteria may have a potential application in fighting Phellinus tremulae, rot-causing fungi pathogenic to aspen [37]. On the basis of these findings, we hypothesize that bacteria may boost SM production in F. excelsior seedlings, thus priming the tree’s metabolism and facilitating higher levels of resilience to H. fraxineus. Hence, this study aimed to assess the ability of Paenibacillus sp. and Pseudomonas sp. bacteria to regulate morphogenetic processes and activate protective SMs synthesis in three different European ash genotypes in vitro. This pilot study evaluates the possibilities of using plant-associated bacteria to improve the quality and resistance of forest replanting material.

2. Materials and Methods

2.1. Ash Genotypes

Seeds of three different genetic families of European ash were collected from a second-generation ash seed orchard in the Vytėnai regional division (Kaunas district, Lithuania) and Ubiškės regional division (Telšiai district, Lithuania). The origin sites of the genotypes are shown in Figure 1.

2.2. Microorganisms

Two different strains of bacteria were used—Paenibacillus sp. (closely related to P. tundrae, 99.06% Identity) and Pseudomonas sp. (closely related to Ps. oryzihabitans, 99.46% Identity). Both were isolated from aspen in vitro cultures. The isolation and identification of the bacteria were described previously [37]. Both bacterial strains were grown on a solid, low-salt, Lysogeny broth (LB) medium (Duchefa Biochemie, Haarlem, Netherlands) (pH ~ 7.0) at ~25 °C. In vitro cultures of the fungus H. fraxineus were established in LRCAF Forest Institute, using samples from F. excelsior trees in the form of lesions from naturally infected leaf petioles from a 40-year-old ash forest stand, damaged by ADB following the isolation procedure described by Kirisits et al. [45]. For H. fraxineus isolation, 10-mm-long petiole fragments containing pseudosclerotia were surface sterilized in 96% ethanol for 1 min, then in 4% NaOCl for 3 min, and then in 96% ethanol again for 30 s. Distilled water (dH2O) was used for rinsing in between the washing steps. Subsequently, the fragments were dried out for 2 min. Afterwards, pseudosclerotial layers were peeled off using sterile utensils. The remaining samples were placed onto a Petri dish containing sterile Hagem agar (malt extract 4 g/L, yeast extract 1 g/L, glucose 5 g/L, NH4Cl 0.5 g/L, KH2PO4 0.5 g/L, MgSO4·7H2O 0.5 g/L, 1% FeCl3 0.5 mL, 100 ppm thiamin 0.125 mL, dH2O to a liter; pH ~ 5.5) (components purchased from Duchefa Biochemie, Haarlem, The Netherlands). Isolates were grown at room temperature in the dark. All growing mycelium fragments were subsequently reisolated onto fresh Petri dishes with Hagem media. Suspected H. fraxineus isolates were screened and identified microscopically [46,47]. Additionally, further identification was caried out as described by Burokiene et al. [48] using H. fraxineus specific primers.
Fungus H. fraxineus was grown on a solid maltose medium containing maltose (20 g/L), yeast extract (8 g/L), tryptone (6 g/L), glucose (20 g/L) and gelrite (6 g/L) (pH 5.8) (Duchefa Biochemie) at ~25 °C (when not in use, all the microorganisms are kept as a glycerol stock at −20 °C).

2.3. Media

During the study seedlings were grown on Murashige and Skoog (MS) medium including vitamins, containing sucrose (20 g/L) and gelrite (4 g/L) (pH 5.8) (media and supplementary components purchased from Duchefa Biochemie). For the seed germination stage, 27 mL of medium was poured into each Petri dish (15 mm × 90 mm) and for the experiment, 30 mL of medium was poured into each clear plastic container (56 mm × 78 mm).

2.4. Seed Germination

Ash seeds were surface disinfected before planting. Firstly, seeds were placed in a liquid-permeable bag and immersed in 2.5% sodium hypochlorite solution for 10 min. After soaking, the bag was rinsed with warm water. The bag of seeds was then immersed in 75% ethanol for 3 min. Afterwards, the bag was transferred to a sterile Petri dish and filled with sterile distilled water, then subsequently soaked for 3 min (this wash was repeated 3 times in total). Later, the ash seed bag was transferred to a new sterile Petri dish and 0.2% silver nitrate solution was added until the seeds were all immersed. Seeds were soaked for 3 min. The bag with the seeds was then transferred to another Petri dish and soaked in sterile water for 3 min. The disinfected seeds were collected from the bag into a new sterile Petri dish. From here the seeds were taken one by one and, using sterile tweezers and scalpels, the germ was removed from each seed. The isolated embryo was then placed in a Petri dish with MS medium (5 germs per plate).
Germination took 2 weeks. After that, suitable (visually similar) seedlings were chosen for the experiment.

2.5. Inoculation with Bacteria and Fungi

For the first-stage inoculation, a day before the transfer of ash seedlings, the MS medium in the plastic containers was spot-inoculated with one of the bacteria using an inoculation needle with ~1.4 × 106 cfu (colony forming units) of Paenibacillus sp. or ~6.4 × 106 cfu of Pseudomonas sp. The bacteria used were taken from bacterial colonies formed on the surface of solid LB medium from overnight cultures.
The amount of cfu per bacterial scrape was determined in a separate experiment using the serial dilution technique.
The fungus H. fraxineus was used for the second-stage inoculation using a modified method [49]. A 7-mm-diameter sample from the edges of the mycelial growth was taken using a sterile cork borer, transferred to a container with the plant medium and placed in the middle, before the transfer of ash seedlings.
The survival of both bacteria and fungus was determined visually.

2.6. Explants in Bacteria/Fungus Inoculated Medium

Germinated plants from in vitro-germinated embryos (about 10 mm in length) were used as explants. They were planted in plastic containers (three explants in one container) with different experimental variants—control (uninoculated medium) and medium inoculated with either bacterial isolate. In the first culture stage, 84 explants for each variant were used in the experiment for family 64, and 40 explants for each variant for families 87 and 174 each. Plants were kept in a growth chamber for 4 weeks (25/20 °C under a 16/8 h photoperiod, white light, irradiance 30 μmol m−2 s−2).
After four weeks, the morphological parameters (shoot length, largest leaf width) of in vitro-grown plants were recorded and new leaves that had formed at the stage of cultivation with bacteria were harvested for biochemical studies. Then, explants were transferred to fungus-inoculated containers for the second-stage trials. Plants were grown for 4 additional weeks under the same conditions as described previously. Afterwards, plant vegetative growth parameters (rooting, shoot length and largest leaf width) were measured, and leaves were again collected for biochemical studies.
The general scheme of the conducted experiments is shown in Table 1.

2.7. Extract Preparation for Secondary Metabolite Analysis

First, 0.5 mg of fresh leaves were kept at −20 °C until analysis. Then, samples were homogenized using mortar and pestle. Then, the resulting material was shaken with 10 mL methanol (75%) for 24 h at 25 °C with a Kuhner Shaker X electronic shaker (Adolf Kühner AG, Birsfelden, Switzerland) at 150 rpm. The extracts were filtered using Whatman no. 1 filter paper, with a retention of 5–8 µm.

2.8. Quantification of Total Phenolic Compounds

Total phenolic content (TPC) was quantified using the Folin–Ciocalteu reagent per Singleton et al. [50]. Previously prepared extracts (0.1 mL) were mixed with 0.1 mL of the Folin–Ciocalteu reagent (2 N) and 2.5 mL of distilled water (dH2O). After 6 min, 0.5 mL of a 25% (w/v) NaCO3 solution was added to the mixture. This mixture was left at room temperature for 30 min. Then thee absorbance was measured using the Synergy HT Multi-Mode Microplate Reader (BioTek Instruments, Inc., Bad Friedrichshall, Germany) at 760 nm using 75% methanol as a blank. Phenol content was expressed as milligrams of chlorogenic acid per gram of fresh weight of leaves (mg CAE/g). The total phenolics were evaluated using a calibration curve y = 5.5358x − 0.0423 (R2 = 0.9975).

2.9. Quantification of Total Flavonoid Content

The total flavonoid content (TFC) in the extracts was quantified according to Striganavičiūtė et al. [37]. Briefly, the extract (1 mL) was mixed with 0.3 mL of 5% (w/v) NaNO2. After 5 min, 0.5 mL of 2% (w/v) AlCl3 was added. Then after an additional 6 min, the solution was neutralized with 0.5 mL of NaOH (1 M). Absorbance was recorded at 470 nm on the Synergy HT Multi-Mode Microplate Reader (BioTek Instruments, Inc.). TFC was expressed as milligrams of catechin per gram of fresh weight of leaves (mg CE/g). TFC was evaluated using a calibration curve y = 11.616x + 0.0634 (R2 = 0.9983).

2.10. Quantification of Photosynthesis Pigments

First, 0.2 g of fresh leaves was sampled for chlorophyll a and b (chl a and b) and carotenoid assays. For the determination of pigment content, the method described by D. Wettstein was used [51]. Fresh leaf matter was ground in acetone (VWR International, Radnor PA, USA) and filtered through Whatman no. 1 filter paper, with a retention of 5–8 µm. The content of carotenoids and chl a and b (mg/g) were estimated spectrophotometrically using the T80 UV-VIS spectrophotometer (PG Instruments, Leicestershire, UK) at wavelengths of 441, 662 and 644 nm (D), respectively. For the calculation of pigment content, the following models were used:
chl   a   mg / g = 9.784 × D 662 0.990 × D 644 × V P × 1000
Carotenoids   mg / g = 4.695 × D 441 0268 × chl   a + chl   b × V P × 1000
chl   b   mg / g = 21.426 × D 644 4.650 × D 662 × V P × 1000
where V = extract volume (mL) and P = fresh leaf matter (g).

2.11. Statistical Data Analysis

Each measurement for SMs and pigments was calculated as an average of 3 technical replicates and 3 biological relicates. A two-tailed Welch’s t-test, intended to compare samples with possibly unequal variances, was conducted to calculate the probability that the means of the different variants are equal [52] (Microsoft Excel). Experimental variants not infected with the fungus were compared with the control without the fungus, and variants using the fungus were compared with the control variant also infected with the fungus.

3. Results

3.1. Isolation and Identification of H. fraxineus

The isolated fungus from naturally infected F. excelsior trees was identified as H. fraxineus, both by morphological and DNA results (Figure 2).

3.2. Effect of the Studied Microorganisms on Rooting of Different Ash Genotypes

The data analysis showed that different ash genotypes showed different responses to inoculation with studied microorganisms, regarding the percentage of rooted explants in the three investigated F. excelsior genotypes (Table 2).
The data analysis showed that all tested F. excelsior genotypes did not have a positive response to the first-stage and second-stage treatment with either bacterium Pseudomonas sp. or bacterium Paenibacillus sp., in regard to rooting (Table 2). However, genotype 87 differed from two others in its response to the first-stage bacterial inoculation. This genotype showed a negative response to both bacteria. The combination of Pseudomonas sp. and H. fraxineus had a negative effect on rooting for genotype 174.

3.3. Effect of Bacterial Inoculation on Ash Shoot Growth and Leaf Biochemistry

The direct effect of nutrient medium inoculation with Paenibacillus sp. or Pseudomonas sp. bacteria on shoot development of different F. excelsior genotypes is shown in Figure 3 (stage 1). In European ash genotype 64, neither average shoot length (Figure 3a) nor leaf width (Figure 3b) was affected by the Paenibacillus sp. bacteria, while Pseudomonas sp. had a negative effect on shoot length. A different situation was observed for genotype 87, where the shoot and leaf development parameters were significantly decreased by both bacteria. In genotype 174, shoot length was negatively affected by Pseudomonas sp. The statistically significant relatively strongest negative impact on shoot length was observed for Pseudomonas sp. bacteria for all tested European ash genotypes (Figure 3a).
The bacterial effects on the chlorophyll pigment contents in F. excelsior leaves are presented in Figure 4. The obtained results show that treatment with both Paenibacillus sp. and Pseudomonas sp. bacterium significantly increased the chlorophyll a/b ratio in genotype 64 (Figure 4a). Meanwhile, the chlorophyll a/b ratio was significantly decreased in response to both bacteria in genotype 87 (Figure 4a), while genotype 174 was not affected.
Similar effects of bacterium Pseudomonas sp., as induced on the chlorophyll a/b ratio, was also found in the carotenoid content (Figure 4b) in European ash genotypes 64 and 87.
However, while Paenibacillus sp. had a negative effect on the carotenoid content in genotype 87, Pseudomonas sp. facilitated a positive increase.
Additionally, with respect to the carotenoid content, the response of European ash genotype 174 to Pseudomonas sp. was different from 64 and 87 genotypes—carotenoid content decreased with Pseudomonas sp. bacterium (Figure 4b).
The TPC (Figure 5a) was highly increased in response to the bacterium Pseudomonas sp. in European ash genotype 87. Meanwhile, the same bacterium had a slight positive effect on total phenol content in genotype 64. Moreover, treatment with Paenibacillus sp. significantly increased the total phenol content in European ash genotypes 64 and 87.
The results on TFC presented in Figure 5b reveal that European ash genotype 87 showed a significantly positive response to bacterium Paenibacillus sp., and genotype 174 showed a positive response to bacterium Pseudomonas sp. Moreover, genotype 64 showed a positive response to both Paenibacillus sp. and Pseudomonas sp. bacteria.

3.4. Long-Term Effect of the Studied Bacteria on Ash Shoot Growth and Leaf Biochemistry after Inoculation with H. fraxineus

The data shown in Figure 6 represents the long-term effect of Paenibacillus sp. or Pseudomonas sp. bacteria on shoot development of different F. excelsior genotypes. The results of second-stage trials were obtained after the explants from the bacterium-inoculated nutrient medium were transferred and cultured on either sterile or fungus-inoculated mediums (stage 2).
It was found that there were no statistically significant differences in average shoot length (Figure 6a), nor leaf width (Figure 6b) in the effect of the bacterium Paenibacillus sp., neither in the sterile second-stage medium nor on the nutrient medium inoculated with H. fraxineus. However, the average shoot parameters in European ash genotype 87 decreased after being inoculated with the bacterium Pseudomonas sp. on the nutrient medium inoculated with H. fraxineus (Figure 6a,b).
Moreover, the Pseudomonas sp. bacterial effect on the leaf development of genotype 87 caused a significant leaf width decrease in both variants (Figure 6b).

3.5. Long-Term Bacterial Inoculation Effect on Ash Leaf Biochemistry after Inoculation with H. fraxineus

The long-term bacterial effects on the chlorophyll and carotenoid content in F. excelsior leaves are shown in Figure 7.
No consistent effect on photosynthetic pigments was observed in either variant. Long-term effects on the chlorophyll a/b ratio of both Paenibacillus sp. and Pseudomonas sp. inoculation were significantly lower in the fungus-free medium of European ash genotype 87. It was observed that the response of genotype 64 to Paenibacillus sp. bacteria was negative, and the response of genotype 174 to the same bacteria was positive (Figure 7a). Moreover, the Pseudomonas sp. bacterial effect on the chlorophyll a/b ratio of genotype 64 caused a significant decrease in the nutrient medium inoculated with H. fraxineus (Figure 7a). Additionally, genotype 174 was negatively affected by H. fraxineus if the explants were inoculated with both bacterium Paenibacillus sp. and Pseudomonas sp.
Long-term bacterial effects on carotenoid content were best seen if the medium of the second stage was not inoculated with H. fraxineus (Figure 7b). It was noted that the long-term effect of Paenibacillus sp. increased carotenoid content in genotypes 64 and 87. Meanwhile, Pseudomonas sp. increased carotenoid content in genotype 64. Only Paenibacillus sp. had a significant effect on carotenoid content in H. fraxineus inoculated shoots; it was positive in genotype 174.
The long-term bacterial effects on SM content (phenols and flavonoids) in F. excelsior leaves are shown in Figure 8.
Paenibacillus sp. and Pseudomonas sp. led to increased concentrations of stress-resilience indicators, including not only previously described carotenoids (Figure 8b) but also phenolic and flavonoid compounds in fungus-free media (Figure 8). In fungus-free genotype 87, TPC increased under the long-term effect of Pseudomonas sp., and decreased in genotype 174 after Paenibacillus sp. treatment (Figure 8a). Both bacteria had a positive effect on TPC of genotype 64 in this variant.
When inoculated with H. fraxineus, Pseudomonas sp. inoculated shoots had higher TPC than their respective controls in European ash genotypes 64 and 87, while in genotype 174 previously inoculated with Paenibacillus sp., TPC significantly decreased. Meanwhile, in seedlings of genotype 87 on the nutrient medium inoculated with H. fraxineus, after the treatment with the Paenibacillus sp. bacterium, TPC increased (Figure 8a).
Both bacteria increased TFC in genotype 64, while Pseudomonas sp. increased it in genotype 87 in fungus-free media; however, after treatment with the Paenibacillus sp. bacterium, TFC decreased in genotypes 87 and 174 in fungus-free media (Figure 8a). A statistically significant increase in TFC was determined in H. fraxineus-inoculated genotypes 64 and 87 after treatment with the Pseudomonas sp. bacterium. Meanwhile, Paenibacillus sp. had a significant positive impact on TFC of genotype 87 on the nutrient medium inoculated with H. fraxineus.

4. Discussion

H. fraxineus causes major damage in European forests, thus the biocontrol of this pathogen is of great importance [53,54]. It has been shown that some European ash genotypes may be somewhat genetically resilient [11,23,24,25,26,27,55,56]. However, we propose that a plant’s secondary metabolism can play a part in ash resistance to H. fraxineus as well. Specifically, the amount of phenolic the trees produce can be used as an indicator [2,57]. Since the production of phenolics is also heritable, genetic selection for the most suitable material for ash reforestation is fitting.
SMs such as phenols and flavonoids are often associated with a plant’s response to both biotic and abiotic stress [28,30,31,32,58,59,60,61]. Higher production of compounds in both of these groups is indicative of systemic resistance due to increases in the chemical defensive response [32,37,62].
Inoculation with microorganisms can influence a plant’s response to varied negative factors [32,37,63,64,65,66,67,68]. Furthermore, microorganisms have an intimate relationship with a plant’s metabolism, possibly serving as regulators of interactions [30]. Thus, in addition to the genetic selection of F. excelsior resilient to H. fraxineus infection, plant-associated bacteria may also be used to boost ash resilience by priming the secondary metabolism apparatus, eliciting induced systemic resistance.
Recent studies have reported ash endophytes that may contribute to tree vitality through antagonisms against H. fraxineus in vitro [21,36,53,69,70].
Moreover, research suggests that bacteria can facilitate enhanced SM production [37,65,71,72,73,74]. Microorganisms affect their host metabolism and protein synthesis in a multitude of ways [75,76], thus pinpointing the exact nature of the bacteria–pathogen–tree interaction is difficult. However, it has been proposed that endophytes may affect a plant’s secondary metabolism in one of three ways: An increase in plant material, which produces the metabolite, the alteration of metabolic pathways or optimization of the production process [77].
During our study, no significant increase in plant morphometric parameters was observed. However, in ash genotype 64, both bacteria elicited an increase in the echlorophyll a/b ratio, carotenoid content, TPC and TFC in the first-stage trial, and carotenoid content, TFC and TPC in the second-stage trials. Moreover, Pseudomonas sp. inoculated seedlings exhibited increased phenolics after H. fraxineus infection too. Increases in chlorophyll content are often linked to enhanced plant health [68,78], while carotenoid content is usually linked to stress, hormone production and antioxidative activity [79,80,81,82,83]. This could potentially indicate that the tested bacteria induce low amounts of stress, thus in return, their host plant upregulates SM production.
Tested bacteria and other ash genotypes did not appear to interact in the same manner as genotype 64. However, in the trial of ash genotype 87, Pseudomonas sp. elicited an increase in TPC and TFC, with or without the additional H. fraxineus infection. Interestingly, it decreased rooting when seedlings were not inoculated with the fungus. Additionally, Paenibacillus sp. also similarly affected family 87, however, only post pathogen infection.
It has been proposed that H. fraxineus attacks European ash at least in part via the phytotoxic metabolite viridiol [55,84]. Cleary et al. found that less-susceptible ash trees had higher amounts of secoiridoids [55]. On the other hand, Nemesio-Gorriz et al. reported it might be coumarins that are responsible for European ash resilience to H. fraxineus [85]. Their research explores the chemical defense of tested trees. They have found that susceptible trees and resilient trees differed in their SM profile. Interestingly, the bark extracts from resilient trees affected the pathogen negatively as did the two isolated coumarins fraxetin and esculetin, which were linked to reduced susceptibility to H. fraxineus. It is possible plant-associated bacteria may upregulate the production of these metabolites (references therein [86]).
Previously, we tested these same bacterial isolates in an analogue experiment on aspen microshoots in vitro using the pathogen Phellinus tremulae—aspen root rot causing fungus [37]. The results were also genotype-dependent, as the effects of both pathogen and tested bacteria varied within a genetic family. It was observed that Pseudomonas sp. affected the morphometric parameters and pigment content of some aspen positively, while Paenibacillus sp. demonstrated a large increase in TPC and TFC in pathogen-infected shoots.
It is also noteworthy that during this study, both Pseudomonas sp. and Paenibacillus sp. affected ash growth negatively, as seen in the rooting data, shoot and leaf growth. This too was noted in our previous study, whereby both bacteria had a negative effect on hybrid aspen and not Populus tremula. In addition, Pseudomonas sp. had a synergistic effect with H. fraxineus—seedlings inoculated with both bacterium and fungus facilitated significantly lower rooting.

5. Conclusions

Bacterial (Pseudomonas sp. and Paenibacillus sp.) interaction with ash (Fraxinus excelsior) seedlings and the pathogenic fungus Hymenoscyphus fraxineus was investigated. Plant-associated bacteria were shown to facilitate increased phenolics and photosynthesis pigment content (Pseudomonas sp. was especially effective), and hence help prime the plants for subsequent pathogenic infection. It is noteworthy that the effect on ash seedlings was dependent on tree genotype, thus demonstrating, in addition to using genetic selection of resilient ash replanting material, utilizing bacteria to boost the production of phenolics is also appropriate.
Future studies will test the effect of ash inoculation under ex vitro conditions, using different inoculation techniques and bacterial concentrations to develop a methodology applicable under field conditions, as well as the identification of specific secondary metabolites.

Author Contributions

Conceptualization, V.S.-Š. and J.Ž.; methodology, V.S.-Š., J.Ž. and D.V.; software, G.S. and D.V.; formal analysis, V.S.-Š., J.Ž. and G.S.; investigation, G.S. and D.V.; resources, J.Ž.; data curation, G.S.; writing—original draft preparation, V.S.-Š., J.Ž., G.S. and D.V.; writing—review and editing, V.S.-Š., J.Ž., G.S. and D.V.; visualization, G.S. and J.Ž.; supervision, V.S.-Š. and J.Ž.; project administration, V.S.-Š. All authors have read and agreed to the published version of the manuscript.

Funding

This research received no external funding.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

Complete study data are available upon request.

Conflicts of Interest

The authors declare no conflict of interest.

References

  1. Sniezko, R.A. Resistance breeding against nonnative pathogens in forest trees—current successes in North America. Can. J. Plant Pathol. 2006, 28, 270–279. [Google Scholar] [CrossRef]
  2. Marčiulynas, A.; Sirgedaitė-Šežienė, V.; Žemaitis, P.; Baliuckas, V. The resistance of Scots pine (Pinus sylvestris L.) half-sib families to Heterobasidion annosum. Forests 2019, 10, 287. [Google Scholar] [CrossRef] [Green Version]
  3. Grulke, N.E. The nexus of host and pathogen phenology: Understanding the disease triangle with climate change. New Phytol. 2010, 189, 9–11. [Google Scholar] [CrossRef] [PubMed]
  4. Pautasso, M.; Dehnen-Schmutz, K.; Holdenrieder, O.; Pietravalle, S.; Salama, N.; Jeger, M.J.; Lange, E.; Hehl-Lange, S. Plant health and global change-some implications for landscape management. Biol. Rev. Camb. Philos. Soc. 2010, 85, 729–755. [Google Scholar] [CrossRef]
  5. FRAXIGEN. Ash Species in Europe: Biological Characteristics and Practical Guidelines for Sustainable Use; University of Oxford: Oxford, UK, 2005; p. 128. [Google Scholar]
  6. Dobrowolska, D.; Hein, S.; Oosterbaan, A.; Wagner, S.; Clark, J.; Skovsgaard, J.P. A review of European ash (Fraxinus excelsior L.): Implications for silviculture. Forestry 2011, 84, 133–148. [Google Scholar] [CrossRef] [Green Version]
  7. Thomas, P.A. Biological Flora of the British Isles: Fraxinus excelsior. J. Ecol. 2016, 104, 1158–1209. [Google Scholar] [CrossRef]
  8. Pautasso, M.; Aas, G.; Queloz, V.; Holdenrieder, O. European ash (Fraxinus excelsior) dieback—A conservation biology challenge. Biol. Conserv. 2013, 158, 37–49. [Google Scholar] [CrossRef]
  9. State Forest Service of Lithuania. Lietuvos Valstybinių Miškų Sanitarinės Būklės Apžvalga, 2020 m; State Forest Service of Lithuania: Kaunas, Lithuania, 2021. [Google Scholar]
  10. Lygis, V.; Bakys, R.; Gustiene, A.; Burokiene, D.; Matelis, A.; Vasaitis, R. Forest self-regeneration following clear-felling of dieback-affected Fraxinus excelsior: Focus on ash. Eur. J. For. Res. 2014, 133, 501–510. [Google Scholar] [CrossRef]
  11. McKinney, L.V.; Nielsen, L.R.; Collinge, D.B.; Thomsen, I.M.; Hansen, J.K.; Kjær, E.D. The ash dieback crisis: Genetic variation in resistance can prove a long-term solution. Plant Pathol. 2014, 63, 485–499. [Google Scholar] [CrossRef]
  12. Latz, M.A.C.; Jensen, B.; Collinge, D.B.; Jorgensen, H.J.L. Endophytic fungi as biocontrol agents: Elucidating mechanisms in disease suppression. Plant Ecol. Divers. 2018, 11, 555–567. [Google Scholar] [CrossRef] [Green Version]
  13. Fadiji, A.E.; Babalola, O.O. Elucidating mechanisms of endophytes used in plant protection and other bioactivities with multifunctional prospects. Front. Bioeng. Biotechnol. 2020, 8, 467. [Google Scholar] [CrossRef] [PubMed]
  14. Glick, B.R. Plant growth-promoting bacteria: Mechanisms and applications. Scientifica 2012, 2012, 963401. [Google Scholar] [CrossRef] [Green Version]
  15. Hossain, M.M.; Sultana, F.; Islam, S. Plant growth-promoting fungi (PGPF): Phytostimulation and induced systemic resistance. In Plant-Microbe Interactions in Agro-Ecological Perspectives; Singh, D., Singh, H., Prabha, R., Eds.; Springer: Singapore, 2017. [Google Scholar] [CrossRef]
  16. Berg, G.; Smalla, K. Plant species and soil type cooperatively shape the structure and function of microbial communities in the rhizosphere. FEMS Microbiol. Ecol. 2009, 68, 1–13. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  17. Berg, G.; Rybakova, D.; Grube, M.; Köberl, M. The plant microbiome explored: Implications for experimental botany. J. Exp. Bot. 2015, 67, 995–1002. [Google Scholar] [CrossRef] [PubMed]
  18. Suman, A.; Yadav, A.N.; Verma, P. Endophytic microbes in crops: Diversity and beneficial impact for sustainable agriculture. In Microbial Inoculants in Sustainable Agricultural Productivity; Singh, D., Singh, H., Prabha, R., Eds.; Springer: New Delhi, India, 2016; Volume 1, pp. 117–143. [Google Scholar] [CrossRef]
  19. Pirttilä, A.M.; Mohammad Parast Tabas, H.; Baruah, N.; Koskimäki, J.J. Biofertilizers and Biocontrol Agents for Agriculture: How to Identify and Develop New Potent Microbial Strains and Traits. Microorganisms 2021, 9, 817. [Google Scholar] [CrossRef] [PubMed]
  20. Terhonen, E.; Blumenstein, K.; Kovalchuk, A.; Asiegbu, F.O. Forest tree microbiomes and associated fungal endophytes: Functional roles and impact on forest health. Forests 2019, 10, 42. [Google Scholar] [CrossRef] [Green Version]
  21. Ulrich, K.; Becker, R.; Behrendt, U.; Kube, M.; Ulrich, A. A Comparative Analysis of Ash Leaf-Colonizing Bacterial Communities Identifies Putative Antagonists of Hymenoscyphus fraxineus. Front. Microbiol. 2020, 11, 966. [Google Scholar] [CrossRef]
  22. McKinney, L.V.; Nielsen, L.R.; Hansen, J.K.; Kjær, E.D. Presence of natural genetic resistance in Fraxinus excelsior (Oleraceae) to Chalara fraxinea (Ascomycota): An emerging infectious disease. Heredity 2011, 106, 788–797. [Google Scholar] [CrossRef] [Green Version]
  23. Pliūra, A.; Lygis, V.; Suchockas, V.; Bartkevičius, E. Performance of twenty four European Fraxinus excelsior populations in three Lithuanian progeny trials with a special emphasis on resistance to Chalara fraxinea. Balt. For. 2011, 17, 17–34. [Google Scholar]
  24. Kjær, E.D.; McKinney, L.V.; Nielsen, L.R.; Hansen, L.N.; Hansen, J.K. Adaptive potential of ash (Fraxinus excelsior) populations against the novel emerging pathogen Hymenoscyphus pseudoalbidus. Evol. Appl. 2012, 5, 219–228. [Google Scholar] [CrossRef]
  25. Stener, L.G. Clonal differences in susceptibility to the dieback of Fraxinus excelsior in southern Sweden. Scand. J. For. Res. 2013, 28, 205–216. [Google Scholar] [CrossRef]
  26. Enderle, R.; Nakou, A.; Thomas, K.; Metzler, B. Susceptibility of autochthonous German Fraxinus excelsior clones to Hymenoscyphus pseudoalbidus is genetically determined. Ann. For. Sci. 2015, 72, 183–193. [Google Scholar] [CrossRef] [Green Version]
  27. Havrdová, L.; Novotná, K.; Zahradník, D.; Buriánek, V.; Pešková, V.; Šrůtka, P. Differences in susceptibility to ash dieback in Czech provenances of Fraxinus excelsior. For. Pathol. 2016, 46, 281–288. [Google Scholar] [CrossRef]
  28. Witzell, J.; Martín, J.A. Phenolic metabolites in the resistance of northern forest trees to pathogens—Past experiences and future prospects. Canadian Journal of Forest Research 2008, 38, 2711–2727. [Google Scholar] [CrossRef]
  29. Li, Y.; Zhang, W.; Sun, N.; Wang, X.; Feng, Y.; Zhang, X. Identification and functional verification of differences in phenolic compounds between resistant and susceptible Populus species. Phytopathology 2020, 110, 805–812. [Google Scholar] [CrossRef] [PubMed]
  30. Pang, Z.; Chen, J.; Wang, T.; Gao, C.; Li, Z.; Guo, L. Linking Plant Secondary Metabolites and Plant Microbiomes: A Review. Front. Plant Sci. 2021, 12, 621276. [Google Scholar] [CrossRef]
  31. Zaynab, M.; Fatima, M.; Abbas, S.; Sharif, Y.; Umair, M.; Zafar, M.H.; Bahadar, K. Role of secondary metabolites in plant defense against pathogens. Microb. Pathog. 2018, 124, 198–202. [Google Scholar] [CrossRef] [PubMed]
  32. Isah, T. Stress and defense responses in plant secondary metabolites production. Biol. Res. 2019, 52, 39. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  33. Sirgedaitė-Šėžienė, V.; Mildažienė, V.; Žemaitis, P.; Ivankov, A.; Koga, K.; Shiratani, M.; Baliuckas, V. Long-term response of Norway spruce to seed treatment with cold plasma: Dependence of the effects on the genotype. Plasma Process. Polym. 2021, 18, 2000159. [Google Scholar] [CrossRef]
  34. Maggini, V.; De Leo, M.; Mengoni, A.; Gallo, E.R.; Miceli, E.; Reidel, R.V.B.; Biffi, S.; Pistelli, L.; Fani, R.; Firenzuoli, F.; et al. Plant-endophytes interaction influences the secondary metabolism in Echinacea purpurea (L.) Moench: An in vitro model. Sci. Rep. 2017, 7, 16924. [Google Scholar] [CrossRef] [PubMed]
  35. Hardoim, P.R.; van Overbeek, L.S.; Berg, G.; Pirttilä, A.M.; Compant, S.; Campisano, A.; Döring, M.; Sessitsch, A. The Hidden World within Plants: Ecological and Evolutionary Considerations for Defining Functioning of Microbial Endophytes. Microbiol. Mol. Biol. Rev. 2015, 79, 293–320. [Google Scholar] [CrossRef] [Green Version]
  36. Becker, R.; Ulrich, K.; Behrendt, U.; Kube, M.; Ulrich, A. Analyzing Ash Leaf-Colonizing Fungal Communities for Their Biological Control of Hymenoscyphus fraxineus. Front. Microbiol. 2020, 11, 590944. [Google Scholar] [CrossRef]
  37. Striganavičiūtė, G.; Žiauka, J.; Sirgedaitė-Šėžienė, V.; Vaitiekūnaitė, D. Impact of Plant-Associated Bacteria on the In Vitro Growth and Pathogenic Resistance against Phellinus tremulae of Different Aspen (Populus) Genotypes. Microorganisms 2021, 9, 1901. [Google Scholar] [CrossRef]
  38. Ulrich, K.; Stauberm, T.; Ewald, D. Paenibacillus—A predominant endophytic bacterium colonising tissue cultures of woody plants. Plant Cell Tissue Organ Cult. 2008, 93, 347–351. [Google Scholar] [CrossRef]
  39. Vaitiekūnaitė, D.; Kuusienė, S.; Beniušytė, E. Oak (Quercus robur) Associated Endophytic Paenibacillus sp. Promotes Poplar (Populus spp.) Root Growth In Vitro. Microorganisms 2021, 9, 1151. [Google Scholar] [CrossRef]
  40. Abdallah, Y.; Yang, M.; Zhang, M.; Masum, M.M.I.; Ogunyemi, S.O.; Hossain, A.; An, Q.; Yan, C.; Li, B. Plant growth promotion and suppression of bacterial leaf blight in rice by Paenibacillus polymyxa Sx3. Lett. Appl. Microbiol. 2019, 68, 423–429. [Google Scholar] [CrossRef] [PubMed]
  41. Egamberdieva, D.; Shurigin, V.; Alaylar, B.; Wirth, S.; Bellingrath-Kimura, S.D. Bacterial endophytes from horseradish (Armoracia rusticana G. gaertn., B. Mey. & Scherb.) with antimicrobial efficacy against pathogens. Plant Soil Environ. 2020, 66, 309–316. [Google Scholar] [CrossRef]
  42. Korejo, F.; Urooj, F.; Farhat, H.; Moin, S.; Viqar, S.; Rahman, A. Effect of soil amendment with Launaea nudicaulis L. on biocontrol potential of endophytic fluorescent Pseudomonas against root rot. Int. J. Biol. Res. 2019, 7, 33–38. [Google Scholar]
  43. Afzal, I.; Shinwari, Z.K.; Iqrar, I. Selective isolation and characterization of agriculturally beneficial endophytic bacteria from wild hemp using canola. Pak. J. Bot. 2015, 47, 1999–2008. [Google Scholar]
  44. Miliute, I.; Buzaite, O.; Gelvonauskiene, D.; Sasnauskas, A.; Stanys, V.; Baniulis, D. Plant growth promoting and antagonistic properties of endophytic bacteria isolated from domestic apple. Zemdirbyste-Agric. 2016, 103, 77–82. [Google Scholar] [CrossRef]
  45. Kirisits, T.; Dampfle, L.; Krautler, K. Hymenoscyphus albidus is not associated with an anamorphic stage and displays slower growth than Hymenoscyphus pseudoalbidus on agar media. For. Pathol. 2013, 43, 386–389. [Google Scholar] [CrossRef]
  46. Halmschlager, E.; Kirisits, T. First report of the ash dieback pathogen Chalara fraxinea on Fraxinus excelsior in Austria. Plant Pathol. 2008, 57, 1177. [Google Scholar] [CrossRef]
  47. Kowalski, T. Chalara fraxinea sp. nov. associated with dieback of ash (Fraxinus excelsior) in Poland. For. Pathol. 2006, 36, 264–270. [Google Scholar] [CrossRef]
  48. Burokiene, D.; Prospero, S.; Jung, E.; Marciulyniene, D.; Moosbrugger, K.; Norkute, G.; Rigling, D.; Lygis, V.; Schoebel, C.N. Genetic population structure of the invasive ash dieback pathogen Hymenoscyphus fraxineus in its expanding range. Biol. Invasions 2015, 17, 2743–2756. [Google Scholar] [CrossRef]
  49. Seppänen, S.K.; Syrjälä, L.; Weissenberg, K.; Teeri, T.H.; Paajanen, L.; Pappinen, A. Antifungal activity of stilbenes in in vitro bioassays and in transgenic Populus expressing a gene encoding pinosylvin synthase. Plant Cell Rep. 2004, 22, 584–593. [Google Scholar] [CrossRef] [PubMed]
  50. Singleton, V.L.; Orthhofer, R.; Lamuela-Raventos, R.M. Analysis of Total Phenols and Other Oxidation Substrates and Antioxidants by Means of Folin-Ciocalteu Reagent. Methods Enzym. 1974, 299, 152–178. [Google Scholar] [CrossRef]
  51. Wettstein, D. Chlorophyll-letale und der submikroskopische Formwechsel der Plastiden. Exp. Cell Res. 1957, 12, 427–506. [Google Scholar] [CrossRef]
  52. Welch, B.L. The Generalization of ‘Students’ Problem when Several Different Population Variances are Involved. Biometrika 1947, 34, 28. [Google Scholar] [CrossRef]
  53. Haňáčková, Z.; Havrdová, L.; Černý, K.; Zahradník, D.; Koukol, O. Fungal endophytes in ash shoots—Diversity and inhibition of Hymenoscyphus fraxineus. Balt. For. 2017, 23, 89–106. [Google Scholar]
  54. Skovsgaard, J.P.; Wilhelm, G.J.; Thomsen, I.M.; Metzler, B.; Kirisits, T.; Havrdova, L.; Enderle, R.; Dobrowolska, D.; Cleary, M.; Clark, J. Silvicultural strategies for Fraxinus excelsior in response to dieback caused by Hymenoscyphus fraxineus. Balt. For. 2017, 90, 455–472. [Google Scholar] [CrossRef] [Green Version]
  55. Cleary, M.R.; Andersson, P.F.; Broberg, A.; Elfstrand, M.; Daniel, G.; Stenlid, J. Genotypes of Fraxinus excelsior with different susceptibility to the ash dieback pathogen Hymenoscyphus pseudoalbidus and their response to the phytotoxin viridiol—A metabolomic and microscopic study. Phytochemistry 2014, 102, 115–125. [Google Scholar] [CrossRef] [PubMed]
  56. Pliūra, A.; Lygis, V.; Marčiulynienė, D.; Suchockas, V.; Bakys, R. Genetic variation of Fraxinus excelsior half-sib families in response to ash dieback disease following simulated spring frost and summer drought treatments. iForest 2016, 9, 12–22. [Google Scholar] [CrossRef] [Green Version]
  57. Bartnik, C.; Nawrot-Chorabik, K.; Woodward, S. Phenolic compound concentrations in Picea abies wood as an indicator of susceptibility towards root pathogens. For. Pathol. 2020, 50, 1–9. [Google Scholar] [CrossRef]
  58. Górniak, I.; Bartoszewski, R.; Króliczewski, J. Comprehensive Review of Antimicrobial Activities of Plant Flavonoids. Phytochem. Rev. 2019, 18, 241–272. [Google Scholar] [CrossRef] [Green Version]
  59. Selmar, D.; Kleinwächter, M. Stress enhances the synthesis of secondary plant products: The impact of stress-related over-reduction on the accumulation of natural products. Plant Cell Physiol. 2013, 54, 817–826. [Google Scholar] [CrossRef] [PubMed]
  60. Kim, Y.; Choi, Y.; Sano, H. Plant vaccination: Stimulation of defense system by caffeine production in planta. Plant Signal. Behav. 2010, 5, 489–493. [Google Scholar] [CrossRef] [Green Version]
  61. Hartmann, T. Plant-derived secondary metabolites as defensive chemicals in herbivorous insects: A case study in chemical ecology. Planta 2004, 219, 1–4. [Google Scholar] [CrossRef]
  62. Wallis, C.M.; Galarneau, E.R.A. Phenolic Compound Induction in Plant-Microbe and Plant-Insect Interactions: A Meta-Analysis. Front. Plant Sci. 2020, 11, 2034. [Google Scholar] [CrossRef]
  63. Pokojska-Burdziej, A.; Strzelczyk, E.; Dahm, H.; Li, C.Y. Effect of Endophytic Bacterium Pseudomonas Fulva on Growth of Pine Seedlings (Pinus sylvestris), Formation of Mycorrhizae and Protection Against Pathogens. Phytopathol. Pol. 2004, 32, 33–47. [Google Scholar]
  64. Naveed, M.; Hussain, M.B.; Zahir, Z.A.; Mitter, B.; Sessitsch, A. Drought stress amelioration in wheat through inoculation with Burkholderia phytofirmans strain PsJN. Plant Growth Regul. 2014, 73, 121–131. [Google Scholar] [CrossRef]
  65. Delaporte-Quintana, P.; Lovaisa, N.C.; Rapisarda, V.A.; Pedraza, R.O. The plant growth promoting bacteria Gluconacetobacter diazotrophicus and Azospirillum brasilense contribute to the iron nutrition of strawberry plants through siderophores production. Plant Growth Regul. 2020, 91, 185–199. [Google Scholar] [CrossRef]
  66. Chakraborty, U.; Chakraborty, B.; Basnet, M. Plant growth promotion and induction of resistance in Camellia sinensis by Bacillus megaterium. J. Basic Microbiol. 2006, 46, 186–195. [Google Scholar] [CrossRef] [PubMed]
  67. Sahu, P.K.; Singh, S.; Gupta, A.R.; Gupta, A.; Singh, U.B.; Manzar, N.; Bhowmik, A.; Singh, H.V.; Saxena, A. Endophytic bacilli from medicinal-aromatic perennial Holy basil (Ocimum tenuiflorum L.) modulate plant growth promotion and induced systemic resistance against Rhizoctonia solani in rice (Oryza sativa L.). Biol. Control 2020, 150, 104353. [Google Scholar] [CrossRef]
  68. Ikram, M.; Ali, N.; Jan, G.; Rahman, I.U.; Iqbal, A.; Hamayun, M. IAA producing fungal endophyte Penicillium roqueforti Thom., enhances stress tolerance and nutrients uptake in wheat plants grown on heavy metal contaminated soils. PLoS ONE 2018, 13, e0208150. [Google Scholar] [CrossRef]
  69. Halecker, S.; Wennrich, J.P.; Rodrigo, S.; Rabsch, L.; Baschien, C.; Steinert, M.; Stadler, M.; Surup, F.; Schulz, B.J. Fungal endophytes for biocontrol of ash dieback: The antagonistic potential of Hypoxylon rubiginosum. Fungal Ecol. 2020, 45, 100918. [Google Scholar] [CrossRef]
  70. Kowalski, T.; Bilanski, P. Fungi Detected in the Previous Year ’ s Leaf Petioles of Fraxinus excelsior and Their Antagonistic Potential against Hymenoscyphus fraxineus. Forests 2021, 12, 1412. [Google Scholar] [CrossRef]
  71. Nowak, J. Benefits of in vitro “biotization” of plant tissue cultures with microbial inoculants. In Vitro Cell. Dev. Biol.-Plant 1998, 34, 122–130. [Google Scholar] [CrossRef]
  72. Grover, M.; Ali, S.Z.; Sandhya, V.; Rasul, A.; Venkateswarlu, B. Role of microorganisms in adaptation of agriculture crops to abiotic stresses. World J. Microbiol. Biotechnol. 2011, 27, 1231–1240. [Google Scholar] [CrossRef]
  73. Zhang, F.S.; Lv, Y.L.; Zhao, Y.; Guo, S.X. Promoting role of an endophyte on the growth and contents of kinsenosides and flavonoids of Anoectochilus formosanus Hayata, a rare and threatened medicinal Orchidaceae plant. J. Zhejiang Univ. Sci. B 2013, 14, 785–792. [Google Scholar] [CrossRef] [Green Version]
  74. Chandrasekaran, M.; Chun, S.C.; Oh, J.W.; Paramasivan, M.; Saini, R.K.; Sahayarayan, J.J. Bacillus subtilis CBR05 for Tomato (Solanum lycopersicum) Fruits in South Korea as a Novel Plant Probiotic Bacterium (PPB): Implications from total phenolics, flavonoids, and carotenoids content for fruit quality. Agronomy 2019, 9, 838. [Google Scholar] [CrossRef] [Green Version]
  75. Mahmood, A.; Kataoka, R. Metabolite profiling reveals a complex response of plants to application of plant growth-promoting endophytic bacteria. Microbiol. Res. 2020, 234, 126421. [Google Scholar] [CrossRef]
  76. Tamošiūnė, I.; Stanienė, G.; Haimi, P.; Stanys, V.; Rugienius, R.; Baniulis, D. Endophytic Bacillus and Pseudomonas spp. Modulate Apple Shoot Growth, Cellular Redox Balance, and Protein Expression Under in Vitro Conditions. Front. Plant Sci. 2018, 9, 889. [Google Scholar] [CrossRef] [Green Version]
  77. Ludwig-Müller, J. Plants and endophytes: Equal partners in secondary metabolite production? Biotechnol. Lett. 2015, 37, 1325–1334. [Google Scholar] [CrossRef]
  78. Kumari, M.; Thakur, I.S. Biochemical and proteomic characterization of Paenibacillus sp. ISTP10 for its role in plant growth promotion and in rhizostabilization of cadmium. Bioresour. Technol. Rep. 2018, 3, 59–66. [Google Scholar] [CrossRef]
  79. Kumar, V.; Kumar, M.; Sharma, S.; Prasad, R. Probiotics Plant Health; Springer: Singapore, 2017. [Google Scholar] [CrossRef]
  80. Havaux, M. Carotenoid oxidation products as stress signals in plants. Plant J. 2014, 79, 597–606. [Google Scholar] [CrossRef]
  81. Cazzonelli, C.I. Carotenoids in nature: Insights from plants and beyond. Funct. Plant Biol. 2011, 38, 833–847. [Google Scholar] [CrossRef] [Green Version]
  82. DellaPenna, D. Carotenoid synthesis and function in plants: Insights from mutant studies in Arabidopsis. Pure Appl. Chem. 1999, 71, 2205–2212. [Google Scholar] [CrossRef]
  83. Nisar, N.; Li, L.; Lu, S.; Khin, N.C.; Pogson, B.J. Carotenoid metabolism in plants. Mol. Plant 2015, 8, 68–82. [Google Scholar] [CrossRef] [Green Version]
  84. Masi, M.; Di Lecce, R.; Tuzi, A.; Linaldeddu, B.T.; Montecchio, L.; Maddau, L.; Evidente, A. Hyfraxinic Acid, a Phytotoxic Tetrasubstituted Octanoic Acid, Produced by the Ash (Fraxinus excelsior L.) Pathogen Hymenoscyphus fraxineus Together with Viridiol and Some of Its Analogues. J. Agric. Food Chem. 2019, 67, 13617–13623. [Google Scholar] [CrossRef] [PubMed]
  85. Nemesio-Gorriz, M.; Menezes, R.C.; Paetz, C.; Hammerbacher, A.; Steenackers, M.; Schamp, K.; Hofte, M.; Svatoš, A.; Gershenzon, J.; Douglas, G.C. Canditate metabolites for ash dieback tolerance in Fraxinus excelsior. J. Exp. Bot. 2020, 71, 6074–6083. [Google Scholar] [CrossRef] [PubMed]
  86. Stringlis, I.A.; De Jonge, R.; Pieterse, C.M.J. The Age of Coumarins in Plant-Microbe Interactions. Plant Cell Physiol. 2019, 60, 1405–1419. [Google Scholar] [CrossRef] [PubMed] [Green Version]
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Figure 1. Map of Lithuania showing the seed orchard (marked with ∆SO1 for 174 and 87 genetic families and ∆SO2 for the 64 genetic family on the map) and origin sites of the genotypes (marked with an asterisk on the map) used for the study. The origin site of the 64 genetic family cannot be identified.
Figure 1. Map of Lithuania showing the seed orchard (marked with ∆SO1 for 174 and 87 genetic families and ∆SO2 for the 64 genetic family on the map) and origin sites of the genotypes (marked with an asterisk on the map) used for the study. The origin site of the 64 genetic family cannot be identified.
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Figure 2. Fungus Hymenoscyphus fraxineus: (a) In a pure culture on maltose nutrient medium; (b) with ash microshoots post inoculation.
Figure 2. Fungus Hymenoscyphus fraxineus: (a) In a pure culture on maltose nutrient medium; (b) with ash microshoots post inoculation.
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Figure 3. Average shoot length (a) and leaf width (b) of different ash genotypes (64, 87 and 174), inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria. Statistically significant differences from the bacterium-free control variant are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
Figure 3. Average shoot length (a) and leaf width (b) of different ash genotypes (64, 87 and 174), inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria. Statistically significant differences from the bacterium-free control variant are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
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Figure 4. Average chlorophyll a/b ratio (a) and carotenoid content (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), inoculated with Paenibacillus sp. and Pseudomonas sp. bacteria. Statistically significant differences from the bacterium-free control variant are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
Figure 4. Average chlorophyll a/b ratio (a) and carotenoid content (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), inoculated with Paenibacillus sp. and Pseudomonas sp. bacteria. Statistically significant differences from the bacterium-free control variant are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
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Figure 5. Average TPC (a) and TFC (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), inoculated with Paenibacillus sp. and Pseudomonas sp. bacteria. Statistically significant differences from the bacterium-free control variant are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
Figure 5. Average TPC (a) and TFC (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), inoculated with Paenibacillus sp. and Pseudomonas sp. bacteria. Statistically significant differences from the bacterium-free control variant are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
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Figure 6. Average shoot length (a) and leaf width (b) of different F. excelsior genotypes (64, 87 and 174), of which explants were first cultured on the nutrient medium inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria, then transferred onto fresh nutrient medium, either sterile (‘Hf−’) or inoculated with the fungus H. fraxineus (‘Hf+’). Statistically significant differences from the control variant, which was not treated with bacteria during the first culture stage, are indicated (for each genotype separately): ** p < 0.01; *** p < 0.001.
Figure 6. Average shoot length (a) and leaf width (b) of different F. excelsior genotypes (64, 87 and 174), of which explants were first cultured on the nutrient medium inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria, then transferred onto fresh nutrient medium, either sterile (‘Hf−’) or inoculated with the fungus H. fraxineus (‘Hf+’). Statistically significant differences from the control variant, which was not treated with bacteria during the first culture stage, are indicated (for each genotype separately): ** p < 0.01; *** p < 0.001.
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Figure 7. Average chlorophyll a/b ratio (a) and carotenoid content (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), of which explants were first cultured on the nutrient medium inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria, then transferred onto fresh nutrient medium, either sterile (‘Hf−’) or inoculated with the fungus H. fraxineus (‘Hf+’). Statistically significant differences from the control variant, which was not treated with bacteria during the first culture stage, are indicated (for each genotype separately): * p < 0.05, ** p < 0.01, *** p < 0.001.
Figure 7. Average chlorophyll a/b ratio (a) and carotenoid content (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), of which explants were first cultured on the nutrient medium inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria, then transferred onto fresh nutrient medium, either sterile (‘Hf−’) or inoculated with the fungus H. fraxineus (‘Hf+’). Statistically significant differences from the control variant, which was not treated with bacteria during the first culture stage, are indicated (for each genotype separately): * p < 0.05, ** p < 0.01, *** p < 0.001.
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Figure 8. Average TPC (a) and TFC (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), of which explants were first cultured on the nutrient medium inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria, then transferred onto fresh nutrient medium, either sterile (‘Hf−’) or inoculated with the fungus H. fraxineus (‘Hf+’). Statistically significant differences from the control variant, which was not treated with bacteria during the first culture stage, are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
Figure 8. Average TPC (a) and TFC (b) in the leaves of different F. excelsior genotypes (64, 87 and 174), of which explants were first cultured on the nutrient medium inoculated with Paenibacillus sp. or Pseudomonas sp. bacteria, then transferred onto fresh nutrient medium, either sterile (‘Hf−’) or inoculated with the fungus H. fraxineus (‘Hf+’). Statistically significant differences from the control variant, which was not treated with bacteria during the first culture stage, are indicated (for each genotype separately): * p < 0.05; ** p < 0.01; *** p < 0.001.
Microorganisms 09 02504 g008
Table
Table 1. Scheme of the inoculation experiments with different microorganisms (bacteria Paenibacillus sp. and Pseudomonas sp. and fungus, Hymenoscyphus fraxineus) during two culturing stages.
Table 1. Scheme of the inoculation experiments with different microorganisms (bacteria Paenibacillus sp. and Pseudomonas sp. and fungus, Hymenoscyphus fraxineus) during two culturing stages.
Experimental VariantFirst Culture Stage
(Four Weeks)		Second Culture Stage
((Four Weeks)
Control--
+Hf.-H.fraxineus
PaenPaenibacillus sp.-
Paen + HfPaenibacillus sp.H.fraxineus
PseuPseudomonas sp.-
Pseu + HfPseudomonas sp.H.fraxineus
Table
Table 2. Percentage of rooted explants in the in vitro cultures of three Fraxinus excelsior genotypes after second stage of culturing with different microorganisms. In the first stage, the nutrient medium was inoculated with either Paenibacillus sp. (‘Paen’) or Pseudomonas sp. (‘Pseu’) bacteria. For the second stage, explants from each variant were transferred onto fresh medium, either sterile or inoculated with fungus H. fraxineus (‘+Hf’). The control group of explants was cultured on sterile media during both stages.
Table 2. Percentage of rooted explants in the in vitro cultures of three Fraxinus excelsior genotypes after second stage of culturing with different microorganisms. In the first stage, the nutrient medium was inoculated with either Paenibacillus sp. (‘Paen’) or Pseudomonas sp. (‘Pseu’) bacteria. For the second stage, explants from each variant were transferred onto fresh medium, either sterile or inoculated with fungus H. fraxineus (‘+Hf’). The control group of explants was cultured on sterile media during both stages.
Experimental VariantEuropean Ash (Fraxinus excelsior L.)
6487174
Control56.52 ± 10.5791.67 ± 8.33100 ± 0
+Hf58.82 ± 12.3066.67 ± 12.60100 ± 0
Paen77.78 ± 10.0850 ± 13.87 *70 ± 15.28
Paen + Hf62.50 ± 10.0977.78 ± 14.9972.73 ± 14.08
Pseu80.95 ± 8.7857.14 ± 13.73 *66.67 ± 16.67
Pseu + Hf91.30 ± 6.0161.11 ± 11.8260 ± 16.33 *
Statistically significant differences from the control variant (for each genotype separately) are indicated: * p < 0.05.
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Striganavičiūtė, G.; Žiauka, J.; Sirgedaitė-Šėžienė, V.; Vaitiekūnaitė, D. Priming of Resistance-Related Phenolics: A Study of Plant-Associated Bacteria and Hymenoscyphus fraxineus. Microorganisms 2021, 9, 2504. https://0-doi-org.brum.beds.ac.uk/10.3390/microorganisms9122504

AMA Style

Striganavičiūtė G, Žiauka J, Sirgedaitė-Šėžienė V, Vaitiekūnaitė D. Priming of Resistance-Related Phenolics: A Study of Plant-Associated Bacteria and Hymenoscyphus fraxineus. Microorganisms. 2021; 9(12):2504. https://0-doi-org.brum.beds.ac.uk/10.3390/microorganisms9122504

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Striganavičiūtė, Greta, Jonas Žiauka, Vaida Sirgedaitė-Šėžienė, and Dorotėja Vaitiekūnaitė. 2021. "Priming of Resistance-Related Phenolics: A Study of Plant-Associated Bacteria and Hymenoscyphus fraxineus" Microorganisms 9, no. 12: 2504. https://0-doi-org.brum.beds.ac.uk/10.3390/microorganisms9122504

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