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Article

Impact of Thermotherapy and Short-Term Storage on Quercus robur L. Acorn Mycobiota and Germination

by
Jelena Kranjec Orlović
*,
Damir Drvodelić
,
Marko Vukelić
,
Matea Rukavina
,
Danko Diminić
and
Milan Oršanić
Faculty of Forestry and Wood Technology, University of Zagreb, 10000 Zagreb, Croatia
*
Author to whom correspondence should be addressed.
Forests 2021, 12(5), 528; https://doi.org/10.3390/f12050528
Submission received: 22 March 2021 / Revised: 21 April 2021 / Accepted: 22 April 2021 / Published: 25 April 2021
(This article belongs to the Special Issue Tree Regeneration by Seeds in Natural Forests)
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Abstract

:
When natural regeneration of Quercus robur stands is hampered by an insufficient acorn yield, human assisted sowing of acorns collected in non-affected stands and stored for some period of time is performed. To inhibit the development of fungi and acorn deterioration during storage, thermotherapy is usually applied by submerging acorns for 2.5 h in water heated to 41 °C. This research aimed to test the effect of four thermotherapy treatments of different durations and/or applied temperatures as well as short-term storage at −1 °C or 3 °C on acorn internal mycobiota and germination. Fungal presence in cotyledons was analyzed in 450 acorns by isolation of mycelia on artificial media, followed by a DNA-based identification. Germination of 2000 acorns was monitored in an open field trial. Thermotherapy significantly decreased fungal diversity, while storage at 3 °C increased the isolation frequency of several fungi, mainly Penicillium spp. The most frequently isolated fungi did not show a negative impact on acorn germination after short-term storage. The study confirmed the efficiency of thermotherapy in the eradication of a part of acorn internal mycobiota, but also its effect on the proliferation of fast-colonizing fungi during storage. However, the latter showed to be more stimulated by storage conditions, specifically by storage at 3 °C.

1. Introduction

Quercus robur L. (English oak, pedunculate oak) is one of the most important European tree species both economically and ecologically. It is widespread throughout most of the continent, predominantly in forest stands, where it provides multiple benefits including wood highly valued for construction, fuel or furniture manufacturing, or as a habitat and food source for various animal and fungal species [1,2,3,4]. In the last several decades a number of European countries have reported a decline of Q. robur caused by a synergy of different abiotic and biotic factors [5]. The usual symptoms include increased crown defoliation and tree mortality, which are likely associated with an insufficient acorn yield and the suppression of grown seedlings by more competitive species in unfavorable site conditions. This often leads to impeded natural regeneration [5,6]. Given the more prominent pressure of newly emerging invasive pathogens and pests, such as the oak lace bug (Corythuca arcuata (Say, 1832)), and spread of the already established ones ensuing from global trade and climate change, there is justified concern for the health status and regeneration of natural Q. robur forest stands both in the present and future [7,8].
The difficulties related to impeded natural regeneration caused by an insufficient acorn yield are overcome by collecting seeds from other stands, storing them, and introducing them in the regeneration area by seeding or sowing, or using them for the production of seedlings which can be utilized for the same purpose [9]. The success of such human assisted regeneration and the progress of a future forest stand highly depend on seed quality [10,11]. Important factors that determine the quality of acorns are their size, weight, viability, moisture content, mineral nutrient reserves, levels of insect and fungus damage, and germination [12,13,14,15,16]. Since Q. robur acorns belong to a group of recalcitrant seeds, which are characterized by a high moisture content and sensitivity to desiccation, they are prone to viability loss during storage [17,18]. Several authors agree that Q. robur acorns cannot be stored for longer than one to three years, depending on storage conditions [19,20,21]. The recommended storage temperatures vary between −3 °C and 4 °C and are usually related to other factors, such as oxygen concentrations, type of storage containers, medium used (e.g., dry peat, sawdust, or no medium), seed pretreatment, etc. [18,22,23,24]. The main factor preserving acorn viability during storage is the moisture content, which should be at least 40% [23,25,26].
However, humid conditions suitable for the preservation of viability are conducive to fungal growth, which can again negatively affect acorn viability and the overall quality [19,27]. In general, fungal presence in seeds of forest tree species is known to have adverse effects on seed viability during storage, germination success, and health condition of the related plants in successive developmental stages. However, some fungi act only as endophytes or saprotrophs with no detrimental impact on the seeds or seedlings [28,29,30]. Oak acorns also host diverse mycobiota externally on the shell and internally on the cotyledons, which is shaped by the maternal (mother tree) and environmental effects and interactions with other seed-inhabiting organisms (like insects) [11,31,32,33,34,35]. Some of the fungi which invade oak acorns can act as antagonists of fungal pathogens or as harmless endophytes or saprotrophs [11,27,31]. On the other hand, some of these fungi are reported to initiate premature acorn shedding from a tree, cause acorn decay, and reduce germination ability [11,27,34,35,36,37,38]. The most detrimental fungal pathogen infecting oak acorns in Europe is considered to be Ciboria batschiana, as it causes black rot and mumification, especially during storage [39,40]. Other common pathogenic fungi found in acorns are Apiognomonia quercina, Botrytis cinerea, Schizophyllum commune, Stereum hirsutum, Diaporthe insularis, Phomopsis spp., Fusarium spp., and Ophiostoma spp [11,32,33].
One of the most effective methods to control Ciboria batschiana prior to acorn storage is thermotherapy treatment by hot water. It is usually conducted for 2.5 h at 41 °C [21,27,41,42]. These conditions do not have a negative impact on acorn germination or subsequent seedling growth, but at the same time they are destructive for the fungus [27,42,43]. Although this treatment can affect other pathogens as well, it does not have an eradicative effect on all seed-borne fungi and can potentially increase acorn susceptibility to new fungal invasions during storage, mostly by various Penicillium and Mucor species [44,45,46]. It is even suggested that changes in acorn mycobiota, followed by thermotherapy treatment, may reduce their storability [44]. Higher treatment temperatures or longer duration times may be more effective for a broader range of fungal species, but it is essential to find the optimal conditions that will eradicate or inhibit target organism(s) without reducing acorn quality [45,47]. However, there are only a few available studies on the use of higher temperatures to treat acorns. They deal, for example, with their effect on insect presence and moisture content [48,49]; however, little is known about their impact on general mycobiota.
Given the importance of acorn quality for the success of regeneration of oak forest stands and the great impact of the applied seed pretreatments, the aim of this research was to test the effect of different thermotherapy treatments and short-term storage conditions on the chosen attributes of Quercus robur acorns. The objectives were to: (1) test the impact of different thermotherapy temperatures on acorn germination in controlled conditions; (2) explore the effect of thermotherapy treatments of different temperatures and durations, followed by short-term storage at two different temperatures, on the mycobiota of acorn cotyledons; and (3) determine if the applied thermotherapy and storage conditions influence acorn germination in an open field trial.

2. Materials and Methods

Acorns were collected in October 2017 from the ground in Quercus robur forest stands. The stands are located in Croatia around the Training and Research Forest Centre Lipovljani, which is managed by the University of Zagreb, Faculty of Forestry and Wood Technology (45.3744° N, 16.8208° E). Empty and insect-damaged acorns were excluded from further analyses by water flotation and visual inspection. The acorns were stored at 3 °C in polyvinyl chloride (PVC) bags until analysis.

2.1. Testing of Acorn Germination at Different Temperatures

Temperature impact on germination was tested in controlled conditions on a sample of 300 acorns separated in 10 groups of 30. Every group was treated by thermotherapy at a different temperature, ranging from 42 to 60 °C, raising 2 °C per each group. For this purpose, groups of acorns were placed in separate PVC containers filled with 350 mL of water preheated to the target temperature and incubated for 2.5 h at the same temperature in a growth chamber (Kambič RK-980 CHCO2, Semič, Slovenia).
Germination was expressed as a proportion of acorns (%) in each group which developed into a normal seedling in the monitoring period, which was tested in accordance with ISTA (International Seed Testing Association) rules [50]. A PVC container filled with 1400 mL of heat-sterilized sand moistened with 518 mL of water was prepared for each group of 30 acorns. The pericarp and testa (seed coat) were removed, and acorns were cut-off two-thirds at the side opposite to the radicle, firmly placed on the sand surface and covered with a 1 cm layer of the same sand. The containers were then covered with PVC foil and lid and placed in a growth chamber (Kambič RK-980 CHCO2, Semič, Slovenia) set to the following conditions: constant temperature 20 °C and constant humidity 80%, with 12 h exposure to daylight (13,400–14,000 lux) and 12 h in the dark. Grown seedlings were inspected weekly for a total period of 42 days.

2.2. Thermotherapy Treatment and Storage Conditions

Considering the standardized acorn thermotherapy method applied in most accredited ISTA laboratories in the world, which entails placing the acorns in a water bath at 41 °C for 2.5 h [21] and based on the results of the previously described acorn germination testing, the chosen thermotherapy conditions in this study were 41 and 45 °C, for 2.5 and 5 h at each temperature. For this purpose, 1960 acorns were separated in four groups of 490, which were exposed to four thermotherapy treatments differing in applied temperature and/or duration. Each group was placed in a separate PVC container in 3 L of water preheated to 41 or 45 °C and then incubated in a growth chamber (Kambič RK-980 CHCO2, Semič, Slovenia) at the same temperature for 2.5 or 5 h.
After treatment, acorns were surface dried at room temperature for several hours and then stored in different conditions. Out of the 490 acorns used for each thermotherapy treatment, 90 were separated for the analysis of fungal presence and 400 for the nursery trial. Those planned for the analysis of fungi were further divided in three groups of 30. The first group was analyzed within 24 h from the treatment (no storage), the second one was stored for one month in a laboratory freezer at −1 °C (Pol-Eko-Aparatura ZLN-T 300, Wodzisław Śląski, Poland), and the third group was stored for the same period in a laboratory refrigerator at 3 °C (Kirsch Super-720, Offenburg, Germany). Acorns designated for the nursery trial were separated in two groups of 200, which were stored for a period of two months at −1 °C and at 3 °C (Figure 1). All groups were stored separately in sealed PVC bags.

2.3. Isolation and Identification of Fungi

Fungal mycelia were isolated from 360 acorns treated by thermotherapy and stored at different conditions (Figure 1) and from an additional 90 non-treated acorns that served as a control, of which 30 were processed immediately upon field sampling and quality inspection, 30 were stored at −1 °C, and 30 at 3 °C for a period of one month.
Acorns were surface sterilized in a sodium hypochlorite (NaOCl) solution (1% v/v) for five minutes and rinsed three times in sterile distilled water. The pericarp was then removed and small pieces (5 × 5 mm) of cotyledons taken from the edges of advancing discolorations or necroses if present, or from visually healthy tissue. The pieces were then plated in 90 mm Petri dishes on potato dextrose agar (PDA, Oxoid, Basingstoke, UK) amended with streptomycin sulphate (200 mg/L, Sigma-Aldrich, St. Louis, MO, USA). Petri dishes were incubated in the dark at 20 °C for four weeks and checked daily for fungal growth. The emerging mycelia were subcultured to the PDA medium. Pure cultures were grouped into morphotypes based on mycelium color, structure and growth speed, coloration of agar, and sporulation. At least one isolate of each morphotype group was used for molecular identification.
DNA extraction was performed according to Ježić et al. with modifications [51,52] and PCR amplification was conducted with primers ITS1-F [53] and ITS 4 [54] in 65 µL reactions containing 200 µM deoxyribonucleoside triphosphates, 0.4 µM of each primer, 0.5 U of Taq DNA polymerase (Sigma-Aldrich, St. Louis, MO, USA), 1.5 mM MgCl2, 1x reaction buffer, and 1 µL of DNA template. Cycling conditions were as follows: an initial denaturation at 95 °C for 5 min, 35 cycles of denaturation at 95 °C for 30 s, annealing at 50 °C for 45 s, extension at 72 °C for 90 s, and a final extension step at 72 °C for 5 min. The resulting PCR products were sequenced using the same primers as in the PCR, at the DNA sequencing facility of Macrogen Europe (Amsterdam, Netherlands). After processing raw data using the BioEdit Sequence Alignment Editor v.7.2.5 software [55], sequences were identified by comparison with reference sequences in the National Center for Biotechnology Information (NCBI) GenBank using the Basic Local Alignment Search Tool (BLAST) [56]. Sequences with 99.0–100% similarity were identified to the species level and those with 95.0–98.99% of similarity to the genus level. In cases of ambiguous results for some morphotypes belonging to the genus Penicillium, additional DNA regions were amplified in PCR reactions, depending on each individual morphotype. Translation elongation factor 1-α (TEF1-α) was amplified using primers EF1-1018F and EF1-1620R [57] following the protocol of Rehner and Buckley [58] and the β-tubulin (TUB2) locus was amplified with a primer set Bt2a and Bt2b [59] according to the protocol of Braun et al. [60].
The impact of thermotherapy treatment and storage conditions on the number of isolated mycelia and different fungal taxa per acorn was analyzed using the Kruskal–Wallis test and multiple comparison of mean ranks for all groups post hoc test. Associations of the ten most frequent fungal taxa with treatment and storage conditions were explored using correspondence analysis (CA). Tests were performed in the TIBCO Statistica 13.5.0 software package (TIBCO Software Inc., Palo Alto, CA, USA).

2.4. Nursery Trial

Nursery germination of acorns was monitored in an open field trial conducted in the nursery “Šumski vrt i arboretum” located at the University of Zagreb, Faculty of Forestry and Wood Technology (45.8202° N, 16.0228° E). A total of 2000 acorns were used in the trial; 1600 treated by thermotherapy (Figure 1) and 400 non-treated control ones, half of which were stored at −1 °C and another half at 3 °C. Acorns were sown on 3 May 2018 in 10 blocks corresponding to 10 groups exposed to different thermotherapy and storage conditions (eight treated groups and two control ones) (Figure 2). In each block acorns were sown in 4 rows per 50 at the depth of 5 cm. Prior to sowing, the acorns were treated with contact fungicide (35% copper + 2% zinc).
Grown seedlings were counted after their first emergence, 21 days after sowing (24 May 2018), and again after an additional 42 days of growth (5 July 2018). Nursery germination (%) was expressed as a share of grown seedlings in a total of 200 sown acorns per each block.
Correlation between the number of obtained isolates of the eight most frequent fungal species (which occurred in at least two acorn groups) and the germination proportion of each acorn group was tested in the TIBCO Statistica 13.5.0 software package (TIBCO Software Inc., Palo Alto, CA, USA).

3. Results

3.1. Impact of Temperature on Acorn Germination in Controlled Conditions

Germination of Quercus robur acorns exposed to a thermotherapy treatment at temperatures ranging from 42 to 60 °C was evaluated based on the number of grown seedlings in the monitoring period. On the 7th day of monitoring, there was no seedling growth in any of the 10 groups of acorns treated at different temperatures. The first seedlings were observed on the 14th day of monitoring only in groups treated at 46 and 48 °C. Generally, most of the seedlings emerged in the third week of monitoring (between the 14th and 21st days) in the groups treated at lower temperatures (42, 44, 46, and 48 °C), while in the groups treated at higher temperatures (54, 56, 58, and 60 °C) there was no observed growth in the entire monitoring period (Figure 3). Germination was the highest in the group treated at 46 °C.

3.2. Impact of Thermotherapy and Storage on Acorn Mycobiota

Mycobiota was analyzed in a total of 450 acorns distributed in 15 groups, of which 12 were exposed to different thermotherapy and storage conditions (Figure 1), and three were control groups stored under different conditions (no storage, at −1 °C, and at 3 °C). The analysis resulted in the growth of 1149 mycelia belonging to 46 different fungal taxa. There was not a single acorn without fungal growth in the group treated at 41 °C for 5 h and stored at −1 °C or in any of the groups stored at 3 °C, regardless of the thermotherapy treatment. In all other groups 10 to 53% of acorns did not reveal fungal presence (Figure 4). The highest number of mycelia was isolated from acorns in groups stored at 3 °C, while the highest number of different fungal taxa was found in the control groups (Figure 4).
The Kruskal–Wallis test revealed that thermotherapy treatment conditions had a significant impact on the number of different fungal taxa found per acorn (H (4) = 66.39, p < 0.001) and that storage conditions significantly affected both the number of isolated mycelia (H (2) = 151.93, p < 0.001) and different fungal taxa per acorn (H (2) = 18.85, p < 0.001). Multiple comparison of mean ranks for all groups showed that the number of fungal taxa per acorn was significantly higher in control groups compared to all treated groups (Table 1). According to the same test, a significantly higher number of mycelia per acorn developed in groups stored at 3 °C in comparison with non-stored ones (p < 0.001) and with those stored at −1 °C (p = < 0.001). However, the groups stored at 3 °C exhibited significantly less different fungal taxa per acorn in comparison with the latter two groups (p = 0.001 and p = 0.031, respectively).
The most frequently isolated species were Penicillium glandicola, encompassing 67% of all isolated mycelia and occurring in all 15 acorn groups, and Penicillium glabrum, represented in 15% of all isolates and found in 13 acorn groups. Among the ten most frequently found fungal taxa were also Truncatella angustata, Tubakia dryina, Fusarium solani, Trichoderma citrinoviride, Alternaria alternata, Talaromyces sp., and Fusarium avenaceum, encompassing together 11% of all isolates obtained in the research. The remainder of 36 fungal taxa was present in five or less isolates and occurred in only one or two acorn groups (Appendix A, Table A1).
The correspondence analysis revealed that association of fungal taxa was statistically significant with both acorn storage (X2 = 306.62, df = 18, p < 0.001) and treatment conditions (X2 = 381.93, df = 36, p < 0.001). P. glandicola, F. solani, and Talaromyces sp. were most associated with acorns stored at 3 °C, while P. glabrum, T. citrinoviride, and F. avenaceum were mostly found in non-stored acorns (Figure 5). In regards to thermotherapy treatments, P. glandicola, T. angustata, and T. citrinoviride were more associated with treated acorns; while T. dryina, F. solani, A. alternata, and F. avenaceum with non-treated acorns (Figure 6).

3.3. Impact of Thermotherapy and Storage on Acorn Germination in A Nursery

Nursery germination of thermotherapy treated and control acorns stored under different conditions (at −1 °C or at 3 °C) was monitored on the 21st and 63rd day after sowing. Acorns stored at 3 °C revealed equal or higher germination success in comparison with the ones stored at −1 °C, except in the control. The highest nursery germination (79%) was recorded in a group treated at 41 °C for 5 h and stored at 3 °C. It was generally higher in groups treated at 41 °C in comparison with groups treated at 45 °C (Figure 7).
For the eight most frequent fungal taxa, which occurred in more than two treatment/storage acorn groups, there was no correlation between the number of their isolates and acorn germination in either of the groups sown in a nursery trial (Table 2).

4. Discussion

Thermotherapy is a recommended acorn treatment for the efficient control or eradication of pathogens and pests [41,48,61] and is usually applied before acorn storage. However, it is suggested by some authors that it can have adverse effects on the stored acorns, in terms of inflicting injuries, increasing their susceptibility to ubiquitous fungi, and reducing their viability [39,44,45]. Therefore, this study aimed to test the impact of different thermotherapy treatments followed by a short-term storage on the Quercus robur acorn mycobiota and germination.
The first experiment, which entailed exposing the acorns to different temperatures for 2.5 h, revealed a high or complete lack of germination in groups treated at temperatures above 48 °C. In those treated at 42 to 48 °C, germination varied between 70 and 87%, which is in accordance with other research reporting scarified acorn germination [62,63] and indicates that these treatment temperatures did not adversely affect germination in laboratory conditions. The temperature of 48 °C could thus be determined as the highest applicable temperature for acorn thermotherapy (among the ones used in this research) with no harmful effect on germination. In the groups treated at 46 and 48 °C, the first seedlings emerged 14 days after sowing, one week earlier than in the groups treated at 42 and 44 °C. This suggests the possible positive effects of the higher temperature on the time of germination, although more elaborative studies including acorn quality attributes are required for such a conclusion. Some of the possible explanations include the widely applicable Van’t Hoff’s rule, which states that metabolic activities rise with temperature increase [64], or the potential stimulating effect of heat damage on the faster development of radicle, as was the case with rodent-damaged acorns in the study conducted by Drvodelić and Oršanić [65].
Since the commonly performed thermotherapy treatment (at 41 °C for 2.5 h) can lead to the proliferation of ubiquitous fungal species during acorn storage [39,41,44,45], the second part of this study focused on the impact of different thermotherapy and short-term storage conditions on the internal acorn mycobiota. Generally, among the ten most frequently isolated species were Penicillim glandicola, P. glabrum, Fusarium solani, F. avenaceum, and Alternaria alternata, which was not surprising as members of these genera were reported to be the most common potentially harmful fungi inhabiting Quercus robur acorns in similar studies [11,27,32,33,66]. Several other frequently isolated species in this research were reported as plant pathogens by other authors, although not on oak acorns. Truncatella angustata is confirmed as the causative agent of leaf spots and fruit rot on several woody hosts [67,68,69,70], Tubakia dryina is described as pathogenic on Q. robur petioles and leaves [71], and Diplodia seriata is reported as a pathogen of Vitis vinifera L. and various pome and stone fruit trees and a xylem colonizer in declining oak trees [72,73,74,75]. As these most common fungi were mostly associated with cotyledon discoloration or necroses (personal observation, data not shown), they might play a role in acorn deterioration or viability loss during longer-term storage or storage under more unfavorable conditions. Some of the species, such as P. glandicola, T. angustata, and T. citrinoviride, were shown to be relatively more associated with treated acorns, indicating that thermotherapy favored their spread. The first one was the most numerous fungus isolated in this study, relatively more frequently found on acorns stored at 3 °C, thus confirming previous findings of Penicillium spp. dominance in treated and stored acorns [27,41]. However, the results indicate that all Penicillium spp. do not share such abilities, since the second most frequent species, P. glabrum, did not reveal a notable association with treated acorns in comparison to control ones and was mostly found on non-stored acorns.
The most detrimental fungal pathogen on European oak acorns, Ciboria batschiana, was not identified in this research. Although this could be predicted for the thermotherapy treated acorns, since this procedure successfully eliminates this pathogen [27,41], its absence from control acorns was not expected. The same results were also reported in Turkey [33]. There are several possible explanations for this, such as the fact that infections depend on forest sites and host conditions [11,33], so they might not have been prominent in the sampling area chosen for this research. Although infections can occur in the crown, most of the acorns are invaded while on the ground [32,76], and as the acorns in this research were collected very shortly after shedding, there might not have been enough time for the noticeable infection to occur. With regard to the fact that damaged and empty acorns, with possible advanced progression of the infection were discarded before analysis, that C. batschiana might not have prevailed in this particular sampling location, and that there might not have been enough opportunity for ground infection, it could be that there was no sufficient inoculum for the spread of the fungus inside and among acorns, especially since storage time was relatively short.
Thermotherapy treatment had a significant impact on the acorn mycobiota diversity in this research. Non-treated control acorns were invaded by a significantly higher number of different fungal species in comparison to the treated ones, regardless of the conditions they were stored in (Figure 4, Table 1), thus confirming the efficiency of thermotherapy in the eradication of a part of acorn mycobiota as stated in research by Knudsen et al. [27]. CA also indicated that some species, namely T. dryina, F. solani, A. alternata, and F. avenaceum, were relatively more associated with control acorns (Figure 6). However, the last was the only one completely eradicated already at 41 °C and 2.5 h exposure (Appendix A, Table A1). There were no significant differences in fungal diversity among the treatment groups, suggesting that an increase in the thermotherapy temperature (from 41 to 45 °C) and duration (from 2.5 to 5 h) did not noticeably affect the survival of more persistent fungal species, although there were on average more various species found in acorns treated at 41 °C for 2.5 h in comparison with the other three treatment groups (Figure 4). For example, Fusarium solani, Alternaria alternata, and Talaromyces sp. were not found in acorns treated at 45 °C, while Tubakia dryina was not present in acorns treated at 45 °C and those treated at 41 °C for 5 h (Appendix A, Table A1).
Acorn storage at 3 °C proved to be more favorable for fungal proliferation compared to non-stored acorns and those stored at −1 °C, as it resulted in zero acorns without fungal growth and a significantly higher number of obtained isolates per acorn than in the latter groups. Thermotherapy treatment did not impact the reduction of isolated mycelia, whose number in all groups stored at 3 °C regardless of the treatment conditions, exceeded the number of isolates obtained in the control groups (Figure 4). These results confirm higher susceptibility of thermotherapy treated acorns to the spread of persistent and ubiquitous fungi during storage as reported [27,44,45,46]. However, they also indicate that storage temperature also plays a significant role, as stated by Schröder [77]. This was corroborated by the smaller number of obtained mycelia per acorn in most of the treated groups which were non-stored or stored at −1 °C, compared to control groups stored in the same conditions. Exceptionally, in the group treated at 41 °C for 5 h and stored at −1 °C and in the non-stored group treated at 41 °C for 2.5 h, these numbers were bigger than for related groups of non-treated acorns, because of the higher occurrence of two ubiquitous species, P. glandicola in the former and both P. glandicola and P. glabrum in the latter.
The number of different fungal taxa colonizing thermotherapy treated acorns stored at 3 °C was significantly smaller compared to acorns stored under other conditions, contrary to the control groups where it was somewhat bigger (Figure 4). This indicates that a few eurivalent species that survived the treatment spread more successfully during storage at this temperature and thus suppressed the potential isolation of other species or maybe even their growth in acorns. This was corroborated by the fact that by far the most numerous fungus in this research, P. glandicola, was mostly associated with acorns stored at 3 °C.
The lowest nursery germination of the analyzed acorns was observed in the control group stored at 3 °C (55%), while the highest in the group treated at 41 °C for 5 h (79%). Generally, germination was somewhat higher in the groups treated at 41 °C compared to those treated at 45 °C, especially when comparing treatments conducted for 5 h. Shorter treatment times should thus be considered when higher temperatures are applied, since such conditions did not seem to have an adverse effect on acorn germination in the study by Belletti et al. [48].
In all thermotherapy treated groups, germination was higher than in the control group stored at 3 °C, which revealed the highest fungal diversity in this research. This supports previous findings that thermotherapy increases germination by eradicating some of the pathogenic fungi present in acorns that could potentially spread during storage, especially at temperatures above zero [27,41,44,77]. At the same time, there was no significant correlation between the occurrence of the most frequently isolated fungi and acorn germination proportion, indicating that the presence and spread of the ubiquitous fungi after treatment did not adversely affect germination after short-term storage. Except in the control group, germination was comparable or was somewhat higher in groups stored at 3 °C than in equally treated groups stored at −1 °C, which confirms that the dominantly present fungus P. glandicola, most frequently associated with treated acorns stored at 3 °C, did not have a detrimental impact on acorn germination after short-term storage. However, these findings do not exclude the possibility of a different outcome after storage for a longer time period, as reported for some fungal species in other studies [27,78,79].
Non-treated acorns stored at −1 °C revealed unexpectedly high nursery germination, which could be explained by the impact of other factors which were not taken into consideration in this study. It was noticed that the position of the group in the open-field layout, which was directly associated with the exposition of soil and planted acorns to the sun, had an effect on germination. Four groups which were positioned at the eastern and western edge of the layout (Figure 2), including the control one stored at −1 °C, resulted in higher acorn germination.

5. Conclusions

The first experiment revealed that in order to ensure the normally expected acorn germination, the thermotherapy temperature applied for 2.5 h should not exceed 48 °C.
The treatment temperatures chosen for further analysis were lower, 41 and 45 °C, and half of the treatments were performed for a longer period of time (5 h). The obtained results confirmed a significant impact of hot-water thermotherapy on the reduction of fungal diversity in treated acorns compared to the non-treated ones. However, there was no significant difference among the applied treatments, indicating that the tested increase of temperature and duration did not contribute materially to the elimination of persistent fungi, although a few potentially harmful species, like F. solani, A. alternata, and T. dryina were eradicated only at the 45 °C or during the 5 h treatment duration at 41 °C.
The study confirmed that thermotherapy treatment can bring about the proliferation of a few fast-colonizing fungi during storage, as two of the three most frequently isolated species were shown to be more associated with the treated acorns. However, the results suggest that storage temperatures play a more important role in their spread, as the most dominant species, P. glandicola, occurred more frequently in acorns stored at 3 °C in comparison with other storage conditions. Storage at this temperature was generally more conducive to the spread of the most persistent fungal colonizers, regardless of the thermotherapy treatment applied, as acorn groups stored at 3 °C revealed significantly more isolated mycelia compared to others.
Given the dominant occurrence of P. glandicola, the treated acorns stored at 3 °C harbored the least number of other fungal taxa, which shows the aggressiveness and adaptability of the fungus during colonization of these tissues. Despite its colonizing abilities, P. glandicola did not seem to have a detrimental effect on acorn germination in the nursery, and neither did the other frequently isolated fungi; however, this does not exclude the possibility of their detrimental impacts after a longer-term storage or storage at higher temperatures.
Acorn nursery germination was affected by factors other than thermotherapy and storage conditions; therefore, the obtained results cannot be considered conclusive. Nevertheless, all treated acorn groups showed higher germination compared to the control group stored at 3 °C, thus justifying the use of thermotherapy as acorn pretreatment, especially when storage at higher temperatures is planned. Somewhat lower germination in groups treated at 45 °C compared to those treated at 41 °C suggests that shorter treatment times should be considered when higher temperatures are applied.
This study has confirmed some of the known benefits of the application of thermotherapy, but also some of its drawbacks. Although thermotherapy can indirectly affect acorn storability and germination, storage temperatures and duration also play a significant role.

Author Contributions

Conceptualization, J.K.O. and D.D. (Damir Drvodelić); Data curation, J.K.O. and D.D. (Damir Drvodelić); Formal analysis, J.K.O., M.V., and M.R.; Funding acquisition, M.O.; Methodology, J.K.O. and D.D. (Damir Drvodelić); Project administration, D.D. (Danko Diminić) and M.O.; Supervision, D.D. (Danko Diminić) and M.O.; Validation, D.D. (Danko Diminić) and M.O.; Writing—original draft, J.K.O.; Writing—review and editing, J.K.O. and D.D. (Damir Drvodelić). All authors have read and agreed to the published version of the manuscript.

Funding

This research received no external funding.

Data Availability Statement

Not Applicable.

Acknowledgments

The authors are grateful to the reviewers for their constructive comments which improved the manuscript.

Conflicts of Interest

The authors declare no conflict of interest.

Appendix A

Table
Table A1. Fungal taxa and related number of isolated mycelia from Quercus robur acorns exposed to different thermotherapy (C, T1, T2, T3, and T4) and storage conditions (no storage, at −1 °C, and at 3 °C).
Table A1. Fungal taxa and related number of isolated mycelia from Quercus robur acorns exposed to different thermotherapy (C, T1, T2, T3, and T4) and storage conditions (no storage, at −1 °C, and at 3 °C).
Closest BLAST MatchGenBank Accession No.Control C41 °C, 2.5 h T141 °C, 5 h T245 °C, 2.5 h T345 °C, 5 h T4No.
Isol 1		No.
Gro 2
No−1 °C3 °CNo−1 °C3 °CNo−1 °C3 °CNo−1 °C3 °CNo−1 °C3 °C
Penicillium glandicolaMW540446MW540447262028342711729299141911265012076614
Penicillium glabrumMW540448MW5318791025293273254 2523113 17913
Truncatella angustataMW540450 121 6 12 712 328
Tubakia dryinaMW54045634411 135
Diplodia seriataMW540462 12 3 2 1 95
Fusarium solaniMW540452
MW540453		1 13 1 1 164
Trichoderma citrinovirideMW5404631 22 1 64
Alternaria alternataMW54045737 1 113
Talaromyces sp.MW540451 2 21 232
Fusarium avenaceumMW540454
MW540455		10 3 132
Talaromyces marneffeiMW540464 1 4 52
Cucurbitariaceae sp.MW5404662 1 32
Epicoccum nigrumMW54046812 32
Stereum hirsutumMW540470 2 1 32
Gnomoniopsis sp.MW540473 11 22
Penicillium vulpinumMW540477
MW531882		 1 1 22
Unidentified mycelium 1 12 121
Alternaria sp. 1MW540459 4 41
Didymellaceae sp.MW5404654 41
Alternaria sp. 2MW5404583 31
Cladosporium sp. 1MW5404693 31
Diaporthe sp.MW540471 3 31
Fusarium graminearumMW5404673 31
Unidentified mycelium 2 3 31
Apiognomonia sp.MW540476 2 21
Penicillium concentricumMW540478
MW531881		 2 21
Penicillium polonicumMW540475
MW531880		 2 21
Pleurostoma sp. 1MW540474 2 21
Tubakia iowensisMW540472 2 21
Unidentified mycelium 3 2 21
Alternaria sp. 3MW540460 1 11
Alternaria sp. 4MW540461 1 11
Cladosporium sp. 2MW540486 1 11
Clonostachys roseaMW540489 1 11
Coryneliaceae sp.MW540485 1 11
Pestalotiopsis sp.MW5404791 11
Phaeoacremonium hungaricumMW5404801 11
Phaeoacremonium tuscanicumMW540482 1 11
Pleosporales sp. 1MW540488 1 11
Pleosporales sp. 2MW540484 1 11
Pleurostoma sp. 2MW540481 1 11
Psathyrellaceae sp.MW540487 1 11
Talaromyces minioluteusMW540483 1 11
Unidentified mycelium 4 1 11
Unidentified mycelium 5 1 11
Unidentified mycelium 6 1 11
TOTAL 72729776451203597120443811828671201149
1 Total number of obtained isolates. 2 Number of treatment/storage and control groups in which fungal taxon occurred.

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Figure 1. Scheme of Quercus robur acorn groups exposed to different thermotherapy treatment and storage conditions, used for the analysis of fungal presence, and for the nursery trial (group labels are given in bold, numbers of used acorns are given in brackets in italic).
Figure 1. Scheme of Quercus robur acorn groups exposed to different thermotherapy treatment and storage conditions, used for the analysis of fungal presence, and for the nursery trial (group labels are given in bold, numbers of used acorns are given in brackets in italic).
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Figure 2. Block distribution of Quercus robur acorn groups exposed to different thermotherapy treatment and storage conditions sown in the nursery trial.
Figure 2. Block distribution of Quercus robur acorn groups exposed to different thermotherapy treatment and storage conditions sown in the nursery trial.
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Figure 3. Germination success of Quercus robur acorns treated by thermotherapy for 2.5 h at different temperatures.
Figure 3. Germination success of Quercus robur acorns treated by thermotherapy for 2.5 h at different temperatures.
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Figure 4. Number of obtained fungal taxa, isolated mycelia, and acorns without fungal growth in Quercus robur acorn groups exposed to different thermotherapy treatment and storage conditions.
Figure 4. Number of obtained fungal taxa, isolated mycelia, and acorns without fungal growth in Quercus robur acorn groups exposed to different thermotherapy treatment and storage conditions.
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Forests 12 00528 g005 550
Figure 5. Correspondence analysis map showing association of the 10 most frequent fungal taxa with acorn storage categories (no storage, storage at −1 °C, and storage at 3 °C).
Figure 5. Correspondence analysis map showing association of the 10 most frequent fungal taxa with acorn storage categories (no storage, storage at −1 °C, and storage at 3 °C).
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Forests 12 00528 g006 550
Figure 6. Correspondence analysis map showing association of the 10 most frequent fungal taxa with acorn thermotherapy treatment categories (C = control, T1 = at 41 °C for 2.5 h, T2 = at 41 °C for 5 h, T3 = at 45 °C for 2.5 h, and T4 = at 45 °C for 5 h).
Figure 6. Correspondence analysis map showing association of the 10 most frequent fungal taxa with acorn thermotherapy treatment categories (C = control, T1 = at 41 °C for 2.5 h, T2 = at 41 °C for 5 h, T3 = at 45 °C for 2.5 h, and T4 = at 45 °C for 5 h).
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Forests 12 00528 g007 550
Figure 7. Nursery germination of thermotherapy treated and non-treated (control) acorns stored under different conditions, monitored 21 and 63 days after sowing.
Figure 7. Nursery germination of thermotherapy treated and non-treated (control) acorns stored under different conditions, monitored 21 and 63 days after sowing.
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Table
Table 1. Impact of thermotherapy treatment conditions on the number of obtained fungal taxa per acorn tested with multiple comparison of mean ranks for all groups post hoc test (significant p values among treatments are highlighted in red).
Table 1. Impact of thermotherapy treatment conditions on the number of obtained fungal taxa per acorn tested with multiple comparison of mean ranks for all groups post hoc test (significant p values among treatments are highlighted in red).
Control41 °C, 2.5 h41 °C, 5 h45 °C, 2.5 h45 °C, 5 h
Control <0.001<0.001<0.001<0.001
41 °C, 2.5 h<0.001 1.0000.6000.465
41 °C, 5 h<0.0011.000 0.3450.264
45 °C, 2.5 h<0.0010.6000.345 1.000
45 °C, 5 h<0.0010.4650.2641.000
Table
Table 2. Pearson correlation coefficients and related p values reveal no significant correlation between the number of obtained isolates of the eight most frequent fungal species and acorn germination in groups sown in a nursery trial.
Table 2. Pearson correlation coefficients and related p values reveal no significant correlation between the number of obtained isolates of the eight most frequent fungal species and acorn germination in groups sown in a nursery trial.
Penicillium glandicolaPenicillium glabrumTruncatella angustataTubakia dryinaDiplodia seriataFusarium solaniTrichoderma citrinovirideAlternaria alternata
Germination0.344−0.201−0.329−0.118−0.487−0.438−0.0790.294
p = 0.331p = 0.577p = 0.353p = 0.746p = 0.154p = 0.206p = 0.828p = 0.410
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Kranjec Orlović, J.; Drvodelić, D.; Vukelić, M.; Rukavina, M.; Diminić, D.; Oršanić, M. Impact of Thermotherapy and Short-Term Storage on Quercus robur L. Acorn Mycobiota and Germination. Forests 2021, 12, 528. https://doi.org/10.3390/f12050528

AMA Style

Kranjec Orlović J, Drvodelić D, Vukelić M, Rukavina M, Diminić D, Oršanić M. Impact of Thermotherapy and Short-Term Storage on Quercus robur L. Acorn Mycobiota and Germination. Forests. 2021; 12(5):528. https://doi.org/10.3390/f12050528

Chicago/Turabian Style

Kranjec Orlović, Jelena, Damir Drvodelić, Marko Vukelić, Matea Rukavina, Danko Diminić, and Milan Oršanić. 2021. "Impact of Thermotherapy and Short-Term Storage on Quercus robur L. Acorn Mycobiota and Germination" Forests 12, no. 5: 528. https://doi.org/10.3390/f12050528

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