Figures
Abstract
European ash (Fraxinus excelsior) is currently battling an onslaught of ash dieback, a disease emerging in the greater part of its native area, brought about by the introduction of the ascomycete Hymenoscyphus fraxineus (= Hymenoscyphus pseudoalbidus). The closely-related fungus Hymenoscyphus albidus, which is indigenous to Europe, is non-pathogenic when in contact with F. excelsior, but could pose a potential risk to exotic Fraxinus species. The North American green ash (Fraxinus pennsylvanica) is planted widely throughout Europe and regenerates naturally within this environment but little is known about the susceptibility of this species to ash dieback. We performed wound inoculations with both fungi (nine strains of H. fraxineus and three strains of H. albidus) on rachises and stems of F. excelsior and F. pennsylvanica under field conditions in Southern Poland. Necrosis formation was evaluated after two months on the rachises and after 12 months on the stems. After inoculation of H. albidus, only small lesions (of up to 1.3 cm in length) developed on the F. excelsior and F. pennsylvanica rachises, but with no significant distinction from the controls. Hymenoscyphus albidus did not cause necrotic lesions on the stems of either Fraxinus species. In contrast, H. fraxineus induced necroses on all inoculated rachises of both ash species with mean lengths of 8.4 cm (F. excelsior) and 1.9 cm (F. pennsylvanica). Necroses also developed on all of the inoculated F. excelsior stems (mean length 18.0 cm), whereas on F. pennsylvanica such lesions only occurred on about 5% of the stems (mean length 1.9 cm). The differences between strains were negligible. No necroses were observed on the control plants. Reisolations of H. albidus were only successful in around 8–11% of the cases, while H. fraxineus was reisolated from 50–70% of the inoculated organs showing necrotic lesions. None of the Hymenoscyphus species were isolated from the control plants. Our data confirm H. fraxineus’ high virulence with regards to F. excelsior and demonstrate a low virulence in relation to F. pennsylvanica under field conditions in Poland. Hymenoscyphus albidus did not express any perceivable pathogenicity on both host species.
Citation: Kowalski T, Bilański P, Holdenrieder O (2015) Virulence of Hymenoscyphus albidus and H. fraxineus on Fraxinus excelsior and F. pennsylvanica. PLoS ONE 10(10): e0141592. https://doi.org/10.1371/journal.pone.0141592
Editor: Simon Shamoun, Natural Resources Canada, CANADA
Received: July 7, 2015; Accepted: October 9, 2015; Published: October 30, 2015
Copyright: © 2015 Kowalski et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited
Data Availability: All relevant data are within the paper.
Funding: The study was financially supported by the Polish National Science Centre (http://ncn.gov.pl), grant number DEC-2011/03/B/NZ9/00078 (grant recipient: TK).
Competing interests: The authors have declared that no competing interests exist.
Introduction
The genus Fraxinus comprises 48 tree and shrub species indigenous to the temperate and subtropical regions of the Northern Hemisphere [1]. In Europe, F. excelsior L. is the most widespread native species, while F. angustifolia Vahl and F. ornus L. thrive in Southern Europe. The American green ash (F. pennsylvanica Marsh.) is the most widely distributed ash species in North America and is also frequently planted in Europe where it has become locally naturalized. Green ash is used for ornamental purposes [2, 3], for timber production [4–6], as part of shelterbelts [7], or as an ameliorative pioneer for fostering the establishment of native trees [2]. In some European countries, green ash is considered an invasive tree species, existing mainly in floodplain forests and along rivers [5, 6, 8].
Since the early 1990s, European ash (F. excelsior) has been undergoing dieback on a large scale in Europe, calling into question both the survival and future use of this species [9–12]. The causal agent of this epidemic is the ascomycete Hymenoscyphus fraxineus (T. Kowalski) Baral, Queloz & Hosoya (= Hymenoscyphus pseudoalbidus Queloz et al., anamorph Chalara fraxinea T. Kowalski) [13, 14]. The pathogen was introduced from East Asia where it occurs on Fraxinus mandshurica Rupr. and F. chinensis ssp. rhynchophylla (Hance) E. Murray (syn. F. rhynchophylla Hance) [15–17]. The fungus infects ash leaves by means of ascospores and generates necrotic lesions, as well as causing the shedding of leaves. Ascomata are formed in the leaf litter during the subsequent summer. On susceptible hosts, the fungal mycelium can spread from the petiole into the shoot, where it causes extensive xylem and bark necroses eventually leading to tree mortality [14].
Fraxinus angustifolia Vahl is also affected by the disease, albeit to a lesser extent, whereas F. ornus seems to be largely tolerant to the fungus. For the introduced F. pennsylvanica, field observations of natural infections in several European countries indicated that this species is less susceptible to ash dieback compared to the European species F. excelsior and F. angustifolia [14, 18–20]. This was corroborated by stem inoculations in a phytotrone [21]. However, to our knowledge, no results of field inoculations on F. pennsylvanica have been reported this day.
The ash dieback pathogen, H. fraxineus, is, morphologically speaking, almost indistinguishable from Hymenoscyphus albidus (Roberge ex Gillet) W. Phillips, the existence of which has been known in Europe for over 150 years [22–24]. This species also infects common ash leaves and forms apothecia on the leaf remnants found on the ground through summer; however, it is not regarded as pathogenic [21, 25–27].
Determining whether F. pennsylvanica could replace F. excelsior or not is of great significance to European forestry. In North America, neither H. fraxineus nor H. albidus are currently present, but both fungi could be introduced in future, thus reinforcing the need for the timely provision of data for the purpose of risk assessment. Therefore, the aim of the present study is to determine the virulence (i.e. the degree of pathogenicity) of both Hymenoscyphus species on F. pennsylvanica under field conditions in Poland and to compare it with the interaction of these fungi with F. excelsior.
Materials and Methods
The tests were conducted on an experimental plot in the Stary Sącz Forest District, Southern Poland (49° 33' 83'' N, 20° 39' 35'' E), on five-year-old Fraxinus excelsior seedlings (provenance Poland) and also on those of F. pennsylvanica (provenance unknown). Permission to conduct the field experiments was obtained from the head forester, Mgr inż. Paweł Szczygieł. Inoculations were performed with six and nine H. fraxineus isolates from Southern Poland [28] on stems and rachises, respectively, as well as three isolates of H. albidus from Switzerland ([24], see Table 1). The strains are deposited in the culture collection of the University of Agriculture in Cracow.
All strains were obtained from F. excelsior.
For inoculum production, the fungi were grown for three weeks in darkness at room temperature on malt extract agar (MEA; 20g ⁄ l malt extract, Difco, Sparks, MD, USA; 15g ⁄ l agar, Difco). Subsequently, for H. fraxineus, small sterile ash wood sticks (5 x 2 x 2 mm) were placed on the colonies and incubated for three additional weeks. For H. albidus, which is only known to occur on leaves, fragments of ash rachises of similar size were used. For control inoculations, sterile sticks, which had been incubated on MEA for three weeks, were used.
The stems of the current season’s growth (0.6–0.8 cm thick) were inoculated in late July 2012, as were the rachises in 2012 and 2013 (Table 1). The inoculum was inserted into superficial tissue incisions as described in [29] and covered by parafilmTM (Bemis Company, www.parafilm.com). Control inoculations were made in the same manner with sterile inocula. In total, 36 stems and 54 rachises of each Fraxinus species were inoculated with both species of Hymenoscyphus respectively (Tables 2 and 3).
For H. albidus, 12 replicate inoculations were made per fungal isolate on rachises in 2012 and six in 2013. Stem inoculations were also performed in 12 replications in 2012.
For H. fraxineus, six rachises and stems, respectively, were inoculated with the same fungal strain. Each inoculation was carried out on a different tree.
The symptoms on rachises were assessed after two months and those on the stems after 12 months. The lengths of superficially visible necrotic lesions, minus the length of the inoculation wound, were measured and any instances of fungal fructification were recorded. In cases where the entire distal part of the organ had died off in both the rachises and the stems, only the axial extension of the primary necrosis (identifiable by virtue of its distinguished tissue discoloration and depression) was determined.
Reisolations were attempted from all stems and rachises with necrotic lesions (both fungus and mock inoculated) and from plants where wound closure was incomplete (but showing no bark necroses) within 24 hours of harvesting [29]. Six tissue samples were taken from each necrotic stem or rachis—two from the inoculation site, two from the proximal lesion edge and two from an intermediate position in the distal part of the lesion. In the case of partially closed wounds, the samples were taken from below the wound surface and from green tissues approximately 1.5 cm distal and proximal to the inoculation wound. The samples (size approx. 5 x 2 x 2 mm; in the case of very little necroses consisting of dead and living host tissue) were excised aseptically upon disinfection of the surface with 96% ethanol and upon removal of the superficial tissue. The samples were placed on malt extract agar (MEA) with 200mg/L Tetracycline (Tetracyclinum TZF Polfa, Poland) and incubated at 15°C for at least three weeks and identified morphologically. The isolation from an organ was regarded as positive if the respective fungus grew from at least one tissue sample. In total, 1362 inoculation samples and 168 control samples underwent evaluation.
For statistical purposes, one-way analysis of variance (ANOVA) was used, followed by a HSD Tukey test for variables with homogeneity of variance and, in other cases, the non-parametric multiple comparison Kruskal-Wallis test was utilized (see results). Homogeneity of variance was tested by means of a Levene's test. All statistical calculations were performed using the software STATISTICA, version 10 (www.statsoft.com).
Results
Once F. excelsior and F. pennsylvanica were inoculated with H. albidus and H. fraxineus, necrotic lesions developed around the inoculation wounds in varying degrees depending on the fungal species tested, the ash species in question and the organ inoculated.
Rachis inoculations with H. albidus
On rachises inoculated with H. albidus, we saw necrotic lesions develop on 16.7% of the wounds on F. excelsior and on 33.3% of those on F. pennsylvanica (Table 2). However, the necroses were small in size (up to 1.2 cm long on F. excelsior and 1.3 cm on F. pennsylvanica) (Table 2, Figs 1 and 2). There was no significant difference in lesion length between the tested isolates (Fig 1). Wound closure was complete in 19.4% of the rachises of both Fraxinus species (Fig 2C and 2D). However, in some cases, necroses developed before wound closure could take place (Fig 2F) or, in other cases, were associated with pronounced callus formation (Fig 2G). In the case of F. pennsylvanica, independent of the presence of a necrotic lesion, reddish discoloration of the rachis surface was observed around the wound in 22.2% of inoculations (Fig 2D–2F).
Difference in necrosis length on F. excelsior and F. pennsylvanica rachises two months after inoculation of selected strains of H. fraxineus and H. albidus. Variables with the same letter are not significantly different for p = 0.05 (HSD Tukey post hoc test after ANOVA).
(A) Wound without callus formation and no necrosis, (B) necrotic lesion starting from the distal wound edge, (C) largely closed wound with no discoloration of the surrounding tissue, (D) completely closed wound surrounded by a narrow area of reddish discoloration, (E) partially closed wound surrounded by a pronounced area of reddish discoloration, (F) completely closed wound surrounded by a narrow necrotic lesion, (G) completely closed wound surrounded by an extended necrotic lesion, (H) partially closed wound with limited necrosis next to the margin. Scale bars denote a length of 0.3 cm.
Stem inoculations with H. albidus
Stem inoculation with H. albidus did not produce necrosis on any of the 72 individual trees for either of the two ash species and the inoculation wounds completely or, in some cases partially healed within one year (Fig 3A–3C, Table 3).
(A) Completely closed wound on F. excelsior, (B) partially closed wound on F. excelsior, (C) completely closed wound on F. pennsylvanica, (D) extensive necrosis on F. excelsior, (E) partially closed wound with small necrotic lesion on F. pennsylvanica, (F) completely closed wound on F. pennsylvanica. Scale bars denote a length of 0.5 cm.
Rachis inoculations with H. fraxineus
Hymenoscyphus fraxineus caused large, light to dark brown necrotic lesions to appear on all inoculated F. excelsior rachises (mean length 8.4 cm, maximal length 16.6 cm; Table 2, Fig 4A) without exhibiting significant differences between the isolates (Fig 1) or between the samples from different years. The leaf section distal to the lesion had died off at the time of harvest (two months post inoculation) in 35.2% of the rachises. The extension of the necrosis in both proximal and distal directions varied considerably and, in some cases, ceased upon insertion of leaflet petiolules.
(A) Extensive necrosis on F. excelsior, (B) necrosis on F. pennsylvanica surrounded by reddish discoloration, the wound surface is blackened due to the formation of a pseudosclerotial plate of the fungus, (C) no further growth of the necrosis upon insertion of a petiolule, (D) necrotic lesion surrounded by reddish discoloration, (E) non-necrotic wound without surrounding discoloration, (F) completely closed wound with pycnidia of Phoma sp. on the protruding tissue resulting from the incision, (G) extensive necrotic lesion with some reddish discoloration at the distal and proximal ends. Scale bars denote a length of 0.3 cm.
Similiarly, on F. pennsylvanica, necroses also developed on all inoculated rachises (Fig 4B–4G). However, these lesions were significantly smaller than those seen on F. excelsior (average length 1.9 cm, maximal length 6.2 cm) and considerably larger than those appearing on the control trees (Table 2). Amongst the fungal isolates, strain No. 20018 produced notably longer lesions (HSD Tukey test, p = 0.05) (Fig 1). In a single case, the formation of a pseudosclerotial plate of H. fraxineus (identified by the presence of Chalara phialides) could be observed on the wound surface (Fig 4B). As with F. excelsior, sometimes the spreading of the lesion was interrupted by leaflet insertions (Fig 4C). The rachis necroses on F. pennsylvanica were often (64.8% of cases) encased in a reddish discolored area (Fig 4B and 4D). Occasionally single leaflets distal to the lesion withered and, in one case, the whole distal leaf portion died off.
Stem inoculations with H. fraxineus
Hymenoscyphus fraxineus caused necrotic lesions on all inoculated F. excelsior stems. Their mean length was 18.0 cm, the maximum being 27.9 cm (Table 3, Figs 5 and 3D). As a result of girdling, the entire distal segments died off in 11.1% of the stems. In contrast, only two out of the 36 (5.5%) inoculated F. pennsylvanica plants developed necrotic lesions (mean length 1.9 cm, Figs 5 and 3E, Table 3). In all other cases, the wounds either completely or partly healed (Fig 3F) and the distal part of the shoot remained healthy and unharmed. There was no significant difference between the inoculated trees and the control ones (Table 3). The difference in necrosis length between F. excelsior and F. pennsylvanica was highly significant. With F. pennsylvanica, there was no significant difference between the inoculated trees and the control ones (Table 3).
Difference in necrosis length on Fraxinus excelsior and Fraxinus pennsylvanica stems 12 months after inoculation with selected strains of Hymenoscyphus fraxineus and Hymenoscyphus albidus. Variables with the same letter are not significantly different for p = 0.05 (Kruskal-Wallis test).
Reisolations and controls
H. albidus was only reisolated from some ofvthe inoculated rachises affected by necrosis and from stems showing incomplete wound closure (Table 4) and never from living tissues extending below or above the wound. In contrast, H. fraxineus was detected in the majority of inoculated rachises of both ash species and in the stems of F. excelsior, but only very rarely in the stems of F. pennsylvanica (Table 4). However, fungi of the mitosporic genera Alternaria, Cladosporium, Colletotrichum, Epicoccum, Fusarium, Lecytophora, Phoma and Phomopsis were repeatedly isolated from necrotic areas or asymptomatic tissues adjacent to the wound. Several species (Alternaria, Cladosporium, Phoma, Phomopsis) had sporulated on the dead tissue at the time of sampling (Fig 4F).
None of the Hymenoscyphus species were isolated from any of the mock inoculations, independent of host species and organ (Fig 6). All control wounds had completely healed at the time of evaluation (Table 4, Fig 6).
(A-B) completely closed wounds on F. excelsior, (C) completely closed wound with strong callus formation, surrounded by reddish discoloration on F. pennsylvanica, (D) normal wound closure with no discoloration, (E) same situation as in D, but with localized reddish discoloration, (F) wound closed by means of an inconspicuous callus, no discoloration, (G) completely closed stem wound on F. excelsior, (H) completely closed stem wound on F. pennsylvanica. Scale bars denote a length of 0.3 cm.
Discussion
The presented study confirms the high virulence of H. fraxineus in relation to F. excelsior. Moreover, we detected no difference in virulence among the fungal strains tested on this host. This uniformity could be explained by the limited allelic diversity of the pathogen population in Europe [15, 21]. The fungus infects several Fraxinus species and F. excelsior is known to be particularly susceptible [14, 30–32]. The encounter of an exotic pathogen with a naive (i.e. non-coevolved) host population can result in the emergence of a new lethal disease. Several such events have previously affected forest tree species populations on a large scale, e.g. chestnut canker, Dutch elm disease, sudden oak death and white pine blister rust [33–37]. A very minor proportion of F. excelsior exhibits a tolerance to to ash dieback, thus hope remains for the evolutionary rescue of the host in the long run [32]. However, the introduction of additional fungal alleles from Asia could possibly negate this effect [15].
The formation of necrotic lesions caused by H. fraxineus was repeatedly demonstrated via artificial stem inoculations [19, 29, 38, 39]. We also observed necroses on ash leaf rachises, which led to the dying off of the distal leaf parts, a symptom commonly observed in nature. However, natural infection occurs via ascospores [40] and it is not possible to adequately imitate this process by means of wound inoculations. After ascospore infection, various processes could be considered decisive for disease expression: (i) subtle defense responses of the host during early stages of the infection process and/or (ii) interactions between the pathogen and epiphytic or endophytic leaf colonizers. With our inoculation technique, we focused on capturing the defense capabilities exhibited by the host when confronted with a previously established infection. The fungal metabolites, which are ultimately responsible for necrosis formation, have yet to be defined. Several secondary metabolites of H. fraxineus have been described [26, 41–46], but their role in necrosis formation is as yet unclear. Currently, the only known H. fraxineus phytotoxins—viridiol and 3,4-dimethylpentan-4-olide—are also produced by its non-pathogenic sister species H. albidus [26, 46].
Hymenoscyphus fraxineus induced significantly smaller lesions on F. pennsylvanica compared to those that formed on F. excelsior and our data are well in line with the observations that green ash is significantly less susceptible to ash dieback than F. excelsior. Also, on this host, there were almost no differences in virulence among the fungal strains, only one of the nine strains caused significantly larger necroses (Fig 1). Concerning the susceptibility of F. pennsylvanica to H. fraxineus, only a small number of coincidental observations are available: In Estonia, F. pennsylvanica is affected to a moderate degree [18]. In Austria, dieback of F. pennsylvanica has only been observed sporadically and this species appears to be much more resistant than both F. excelsior and F. angustifolia [20]. In northern Germany, only mild symptoms were noted subsequent to exposure to natural infection pressure [19]. However, following stem wound inoculations with H. fraxineus in a phytotron, F. pennsylvanica exhibited a moderate level of susceptibility. In addition, a relatively high proportion (16% out of 75) of natural stem infections was observed on plants delivered from a nursery in Germany [21]. As a consequence, we cannot discount the importance of environment-related predisposition with regards to this host’s susceptibility [47] or the possibility that particularly susceptible provenances exist [48]. The native range of green ash is vast and the species comprises at least three ecotypes [49]. A significant drawback of our data, as well as of the studies cited above, is the fact that no detailed information on host provenance is available. Future susceptibility tests should therefore be performed on a more representative selection of F. pennsylvanica genotypes.
For F. pennsylvanica, in contrast to F. excelsior, the susceptibility of rachises was much higher than that of stems, but the extension of the necroses along rachises took shape more slowly than they did on F. excelsior, indicating the presence of an effective defense mechanism. Consequently, the risk of stem infection is considerably smaller for F. pennsylvanica than for F. excelsior. This gives rise to the possible solution of replacing, to an extent, infested F. excelsior with F. pennsylvanica in Europe. However, this only applies should the expansion of the emerald ash borer in Europe be contained [50, 51].
Neither H. fraxineus nor H. albidus have been detected in North America [52]. The introduction of H. fraxineus to North America would add to the threat already being posed by the emerald ash borer. Since green ash, like other ash species, could serve as a vector for the ash-dieback pathogen, plant transfer from Europe or Asia to North America should be avoided. Other American ash species are also at risk, such as F. nigra Marsh., which has proven highly susceptible to H. fraxineus in Estonia [18]. Our experiments demonstrate that H. albidus, which is indigenous to Europe, is virtually non-pathogenic for both ash species, independent of the inoculated organ (rachis or stem). Only small necrotic lesions developed on a handful of artificially inoculated ash rachises and H. albidus was seldom reisolated. Consequently, we cannot disregard that H. albidus exerts some influence, albeit minor, on the tissues surrounding the inoculation wound, potentially predisposing them to secondary fungi. albudus
This fungus is evidently particukarly poorly adapted to the wound environment or, alternatively, it does not compete well against other wound colonizing microbes. Hymenoscyphus albidus was never isolated from living tissue and this could cast doubts on the possibility of this species leading an endophytic lifestyle, as suggested by Baral und Bemmann [23]. Nevertheless, molecular detection techniques could possibly reveal the presence of the fungus in living plant tissue, as shown by Cleary et al. [53] for H. fraxineus in ash seeds. So far, F. excelsior rachises (and in rare cases those of F. angustifolia) have been recognized as a substrate of H. albidus [23, 54–56]. The sporulation window of H. albidus spans July to September [23, 56]. Our inoculations were made using colonized rachis pieces at the beginning of this period, most likely providing a suitable precondition for fungal development. In any case, our data show that the ecological behaviour of H. albidus does not mirror that of H. fraxineus after wound inoculation and further detailed studies of its biology are required. In comparison with H. fraxineus, such data might enhance our understanding of ash dieback etiology. In spite of the limitations discussed above, we conclude that H. albidus does not pose a noteworthy risk for F. pennsylvanica and the same has also recently been concluded for F. mandshurica [27]. However, the Hymenoscyphus species comprise only a minute proportion of the whole tree microbiome and ecological surprises could definitely arise [57]. Avoidance of further pathogen introductions and a comprehensive understanding of host-pathogen interactions in a changing environment represent the greatest modern-day challenges for forest pathology [58].
Acknowledgments
The authors express their gratitude to Mgr inż. Paweł Szczygieł (Head of Stary Sącz Forest District) for their help during our research, to Andrin Gross, Lioba Paul, Marco Pautasso, Thomas Sieber and two anonymous reviewers for constructive comments on the manuscript, as well as to Christine Syrad for linguistic corrections.
Author Contributions
Conceived and designed the experiments: TK PB. Performed the experiments: TK PB. Analyzed the data: PB. Wrote the paper: OH TK.
References
- 1. Wallander E (2012) Systematics and floral evolution in Fraxinus (Oleaceae). Belgische Dendrologie Belge 2012: 39–58.
- 2. Kremer D, Čavlović J (2005) Distribution of introduced North American ash species and their role in lowland forest management in Croatia. Journal of Forestry 103 (6): 309–313.
- 3.
Selikhovkin AV, Musolin DL (2013) Pests and diseases of Fraxinus spp. in the Russian Federation. Cost Action FP1103 FRAXBACK, 4th MC Meeting & Workshop "Frontiers in ash dieback research" 4–6 September 2013, Malmö, Sweden, Abstracts p. 26.
- 4.
Klimo E, Hager H (eds) (2001) The floodplain forests in Europe. European Forest Institute, Research Rep.10, Leiden, Boston, Köln, 267 pp.
- 5. Schmiedel D, Huth F, Wagner S (2013) Using data from seed-dispersal modelling to manage invasive tree species: the example of Fraxinus pennsylvanica Marshall in Europe. Environmental Management 52: 851–860. pmid:23974901
- 6. Pyšek P, Sádlo J, Mandák B (2002) Catalogue of alien plants of the Czech Republic. Preslia 74: 97–186.
- 7. Gogin VA (1976) Shelterbelts in the Rostov region. Lesnoe Khozyaistvo 6: 31–33.
- 8.
Tiborcz V, Zagyvai G, Korda M, Schmidt D, Csiszár Á, Šporčić D, et al. (2011) Distribution and significance of some invasive alien woody plant species in Hungary. In: 3rd International Sypmposium on Environmental Weeds and invasive Plants, October 2nd to 7th, 2011, Monte Verità, Switzerland. Retrieved February 08, 2012, from http://www.wsl.ch/epub/ewrs/sessions/posters_EN?ID=11
- 9. Kowalski T (2009) Rozprzestrzenienie grzyba Chalara fraxinea w aspekcie procesu chorobowego jesionu w Polsce [Expanse of Chalara fraxinea fungus in terms of ash dieback in Poland]. Sylwan 153 (10): 668−674.
- 10. Pautasso M, Aas G, Queloz V, Holdenrieder O (2013) European ash (Fraxinus excelsior) dieback—A conservation biology challenge. Biological Conservation 158: 37–49.
- 11. Littlewood NA, Nau BS, Pozsgai G, Stockan JA, Stubbs A, Young MR (2015) Invertebrate species at risk from ash dieback in the UK. Journal of Insect Conservation 19: 75–85.
- 12. Mitchell RJ, Beaton JK, Bellamy PE, Broome A, Chetcuti J, Eaton S, et al. (2014) Ash dieback in the UK: a review of the ecological and conservation implications and potential management options. Biological Conservation 175: 95–109.
- 13. Baral HO, Queloz V, Hosoya T (2014) Hymenoscyphus fraxineus, the correct scientific name for the fungus causing ash dieback in Europe. IMA Fungus 5 (1): 79–80. pmid:25083409
- 14. Gross A, Holdenrieder O, Pautasso M, Queloz V, Sieber TN (2014 a) Hymenoscyphus pseudoalbidus, the causal agent of European ash dieback. Molecular Plant Pathology 15 (1): 5–21. pmid:24118686
- 15. Gross A, Hosoya T, Queloz V (2014 b) Population structure of the invasive forest pathogen Hymenoscyphus pseudoalbidus. Molecular Ecology 23: 2943–2960.
- 16. Gross A, Han J (2015) Hymenoscyphus fraxineus and two new Hymenoscyphus species identified in Korea. Mycological Progress 14: 19,
- 17. Zhao YJ, Hosoya T, Baral HO, Hosaka K, Kakishima M (2012) Hymenoscyphus pseudoalbidus, the correct name for Lambertella albida reported from Japan. Mycotaxon 122: 25–41.
- 18. Drenkhan R, Hanso M (2010) New host species for Chalara fraxinea. New Disease Reports 22: 16.
- 19. Lösing H (2013) Susceptibility of Fraxinus species to ash dieback caused by Chalara fraxinea. Acta Horticulturae 1014: 201–203.
- 20.
Kirisits T (2014) The silvicultural importance and ash dieback susceptibility of Fraxinus species in Austria and recommendations for disease management. COST Action FP1103 FRAXBACK 6th MC Meeting & Workshop, 15-18th of September 2014, Palanga, Lithuania. Abstracts, pp. 8–9.
- 21. Gross A, Sieber TN (2015) Virulence of Hymenoscyphus albidus and native and introduced Hymenoscyphus fraxineus on Fraxinus excelsior and Fraxinus pennsylvanica. Plant Pathology (in press)
- 22. Kowalski T, Holdenrieder O (2009 a) The teleomorph of Chalara fraxinea, the causal agent of ash dieback. Forest Pathology 39: 304–308.
- 23. Baral HO, Bemmann M (2014) Hymenoscyphus fraxineus vs. Hymenoscyphus albidus–A comparative light microscopic study on the causal agent of European ash dieback and related foliicolous, stroma-forming species. Mycology 5 (4): 228–290. pmid:25544935
- 24. Queloz V, Grünig CR, Berndt R, Kowalski T, Sieber TN, Holdenrieder O (2011) Cryptic speciation in Hymenoscyphus albidus. Forest Pathology 41:133–142.
- 25. Husson C, Scala B, Cael O, Frey P, Feau N, Ioos R, et al. (2011) Chalara fraxinea is an invasive pathogen in France. European Journal of Plant Pathology 130: 311–324.
- 26. Citron CA, Junker C, Schulz B, Dickschat JS (2014) A volatile lactone of Hymenoscyphus pseudoalbidus, pathogen of European ash dieback, inhibits host germination. Angewandte Chemie International Edition 53: 4346–4349.
- 27. Gross A, Holdenrieder O (2015) Pathogenicity of Hymenoscyphus fraxineus and H. albidus towards Fraxinus mandshurica var. japonica. Forest Pathology 45: 172–174.
- 28. Kraj W, Kowalski T (2014) Genetic variability of Hymenoscyphus pseudoalbidus dieback cause of European ash (Fraxinus excelsior L.). Journal of Phytopathology 162: 218–227.
- 29. Kowalski T, Holdenrieder O (2009 b) Pathogenicity of Chalara fraxinea. Forest Pathology 39: 1–7.
- 30. Bengtsson SBK, Barklund P, von Brӧmssen C, Stenlid J (2014) Seasonal pattern of lesion development in diseased Fraxinus excelsior infected by Hymenoscyphus pseudoalbidus. PLOS ONE 9 (4): e76429. pmid:24759550
- 31. Kräutler K, Kirisits T (2012) The ash dieback pathogen Hymenoscyphus pseudoalbidus is associated with leaf symptoms on ash species (Fraxinus spp.). Jornal of Agricultural Extension & Rural Development 4 (9): 261–265.
- 32. McKinney LV, Nielsen LR, Collinge DB, Thomsen IM, Hansen JK, Kjaer ED (2014) The ash dieback crisis: genetic variation in resistance can prove a long-term solution. Plant Pathology 63: 485–499.
- 33. Anagnostakis SL (1987) Chestnut blight: the classical problem of an introduced pathogen. Mycologia 79: 23–37.
- 34. Geils BW, Humer KE, Hunt RS (2010) White pines, ribes, and blister rust: a review and synthesis. Forest Pathology 40: 147–185.
- 35. Santini A, Faccoli M (2015) Dutch elm disease and elm bark beetles: a century of association. iForest 8: 126–134.
- 36. Sturrock RN, Frankel SJ, Brown AV, Hennon PE, Kliejunas JT, Lewis KJ, et al. (2011) Climate change and forest diseases. Plant Pathology 60: 133–149.
- 37. Holdenrieder O, Pautasso M, Weisberg PJ, Lonsdale D (2014) Tree diseases and landscape processes: the challenge of landscape pathology. Trends in Ecology and Evolution 19: 446–452.
- 38. Bakys R, Vasaitis R, Barklund P, Ihrmark K, Stenlid J (2009) Investigations concerning the role of Chalara fraxinea in declining Fraxinus excelsior. Plant Pathology 58: 284–292.
- 39. Kräutler K, Treitler R, Kirisits T (2015) Hymenoscyphus fraxineus can directly infect intact current-year shoots of Fraxinus excelsior and artificially exposed leaf scars. Forest Pathology 45: 274–280.
- 40. Cleary MR, Daniel G, Stenlid J (2013) Light and scanning electron microscopy studies of the early infection stages of Hymenoscyphus pseudoalbidus on Fraxinus excelsior. Plant Pathology 62: 1296–1305.
- 41. Grad B, Kowalski T, Kraj W (2009) Studies on secondary metabolite produced by Chalara fraxinea and its phytotoxic influence on Fraxinus excelsior. Phytopathologia 54: 61–69.
- 42. Andersson PF, Johansson SBK, Stenlid J, Broberg A (2010) Isolation, identification and necrotic activity of viridiol from Chalara fraxinea, the fungus responsible for dieback of ash. Forest Pathology 40: 43–46.
- 43. Andersson PF, Bengtsson S, Stenlid J, Broberg A (2012) B-norsteroids from Hymenoscyphus pseudoalbidus. Molecules 17: 7769–7781. pmid:22732888
- 44. Andersson PF, Bengtsson S, Cleary M, Stenlid J, Broberg A (2013) Viridin-like steroids from Hymenoscyphus pseudoalbidus. Phytochemistry 86: 195–200. pmid:23098903
- 45. Cleary MR, Andersson PF, Broberg A, Elfstrand M, Daniel G, Stenlid J (2014) 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 102: 115–125. pmid:24709032
- 46. Junker C, Mandey F, Pais A, Ebel R, Schulz B (2014) Hymenoscyphus pseudoalbidus and Hymenoscyphus albidus: viridiol concentration and virulence do not correlate. Forest Pathology 44: 39–44.
- 47. Bostock RM, Pye MF, Roubtsova TV (2014) Predisposition in plant disease: exploiting the nexus in abiotic and biotic stress perception and response. Annual Review of Phytopathology 52: 517–549. pmid:25001451
- 48. Hausman CE, Bertke MM, Jaeger JF, Rocha OJ (2014) Genetic structure of green ash (Fraxinus pennsylvanica): implications for he establishment of ex situ conservation protocols in light of the invasion of the emerald. Plant Genetic Resources: Characterization and Utilization 12 (3): 286–297.
- 49.
Kennedy HE (1990) Green ash. In: Silvics of North America, Vol 2 Hardwoods (ed. by Burns RM and Honkala BH. USDA Forest Service, Agriculture Handbook 654 retrieved September 25, 2015 from http://www.na.fs.fed.us/pubs/silvics_manual/volume_2/fraxinus/pennsylvanica.htm
- 50. Orlova-Bienkowskaja MJ (2014) Ashes in Europe are in danger: the invasive range of Agrilus planipennis in European Russia is expanding. Biological Invasions 16 (7): 1345–1349.
- 51. Valenta V, Moser D, Kuttner M, Peterseil J, Essl F (2015) A high-resolution map of emerald ash borer invasion risk for southern central Europe. Forests 2015 (6): 3075–3086.
- 52.
Farr DF, Rossman, AY (2015) Fungal Databases, Systematic Mycology and Microbiology Laboratory, ARS, USDA. Retrieved September 25, 2015, from http://nt.ars-grin.gov/fungaldatabases/
- 53. Cleary MR, Arhipova N, Gaitnieks T, Stenlid J, Vasaitis R (2013) Natural infection of Fraxinus excelsior seeds by Chalara fraxinea. Forest Pathology 43: 83–85.
- 54.
Rehm H (1896) Ascomyceten: Hysteriaceen und Discomyceten. In: Kryptogamen-Flora von Deutschland, Ӧsterreich und der Schweiz. Bd. 3, ed by Rabenhorst GL, Leipzig: Eduard Kummer, 1275 S.
- 55.
Ellis MB, Ellis JP (1985) Microfungi on Land Plants. Slough: Richmond Publ., 868 pp.
- 56.
Breitenbach J, Krӓnzlin F (1984) Fungi of Switzerland, Vol. 1 Ascomycetes. Lucerne: Mycological Society of Lucerne, 310 pp.
- 57. Lindenmayer DB, Likens GE, Krebs CJ, Hobbs RJ (2010) Improved probability of detection of ecological "surprises". Proceedings of the National Academy of Sciences of the United States of America 107: 21957–21962. pmid:21098660
- 58. Pautasso M, Schlegel M, Holdenrieder O (2015) Forest health in a changing world. Microbial Ecology 69: 826–842. pmid:25502075