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iForest - Biogeosciences and Forestry

iForest - Biogeosciences and Forestry
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Brown rot on nuts of Castanea sativa Mill: an emerging disease and its causal agent

iForest - Biogeosciences and Forestry, Volume 6, Issue 5, Pages 294-301 (2013)
doi: https://doi.org/10.3832/ifor0952-006
Published: Jul 16, 2013 - Copyright © 2013 SISEF

Research Articles

The quality and quantity of nut production are fundamental to the economic viability of chestnut cultivation, yet recent reports indicate that severe damage due to moulds represents a significant problem for growers. We carried out an investigation of the agents of chestnut rot and internal fruit damage in three orchards in Italy. Black and brown rot, as well as insect damage, were found in all the areas examined. Brown rot appeared to be the main cause of damage, affecting 8% to 49% and 2% to 24% of nuts collected from the ground and from burrs, respectively. With respect to morphology and DNA sequencing analyses, fungal isolates obtained from brown rot were homologous with Gnomoniopsis sp. obtained from Dryocosmus kuriphilus (Yasumatsu) galls and with Gnomoniopsis castanea and Gnomoniopsis smithogilvyi described on chestnut in Italy and Australia, respectively. The same fungus was also isolated from the bark of one- and two-years-old healthy shoots at each site, supporting the endophytic behaviour of this rot agent. Brown rot symptoms on nuts associated with Gnomoniopsis sp. corresponded with those previously described by several authors and referred to as Phoma or Phomopsis endogena, suggesting a relationship between these fungi and Gnomoniopsis sp. It is to notice that the escalation of brown rot damage in Italy followed several periods of drought and probably the recent invasion of D. kuriphilus, both stress factors for chestnut trees.

Nut mould, Gnomoniopsis sp., endophytism

  Introduction 

Chestnut cultivation has progressed in Italy and other European countries as a result of a favourable market and the recovery of trees following natural establishment of hypovirulence in chestnut blight ([40]). Chestnut orchards and stands are still vital to the economy of many mountain communities as elements of the landscape, sources of timber and, in particular, for the production of nuts. The quality of chestnuts is determined by size, shape, color, flavor and texture, features which are very important for both fresh consumption and processing ([15]) and which are essential to ensuring an advantageous income for growers. These fruits contain sugars, especially monosaccharides and disaccharides such as sucrose, glucose, fructose and raffinose, as well as starch ([2]). As a consequence, they are highly attractive to insects and fungi, which can cause severe damage and hence pose a considerable problem for chestnut cultivation. Attacks by insect larvae (e.g., Cydia splendana Hb., Cydia fagiglandana Zell. and Curculio elephans Gyll.) are well known to be detrimental to the harvesting of healthy chestnut fruits ([21] ). Several fungi are also capable of colonizing nuts and causing damage: Phoma endogena Speg. and Phomopsis endogena Speg. Cif. have been described as agents of brown rot, Sclerotinia pseudotuberosa Rehm (syn. Ciboria batschiana Zopf) can cause black rot, while Penicillium spp. and Penicillium crustaceum L. Fr. produce greenish moulds. Environmental factors can also influence the quality of fruits ([12]): low soil water availability and high temperatures are destabilizing factors for normal chestnut growth as they are responsible for decreased plant vigor and sub-standard fruit production and also exacerbate the effect of pest and fungi damage ([14], [9]).

The recent appearance of the invasive Asian chestnut gall wasp (Dryocosmus kuriphilus Yasumatsu) in Italian chestnut stands and orchards is causing new concern for the sustainability of chestnut cultivation ([4]). An unusual level of fruit damage was reported in Piedmont, more or less in correspondence with the wasp invasion, ([13]) and subsequently in other chestnut-producing areas of Italy, such as Trentino, Emilia Romagna, Tuscany, Lazio and Campania (Maresi, Poli & Sigillo, personal comm.). The damage in Piedmont was initially attributed to in Gnomonia pascoe ([13]) and recently related to Gnomoniopsis castanea, a proposed new species ([43]). Attacks of brown rot have also occurred in chestnut cultivations in Australia, where the agent was identified as Gnomoniopsis smithogilvyi ([31]). Gnomoniopsis sp. has been found to be associated with necrosis of D. kuriphilus galls ([17]), raising interest in its use as a biocontrol agent against this hymenopteran ([41]).

In this study, we investigated brown rot damage reported in three different Italian chestnut-growing areas in Piedmont, Trentino and Tuscany with the aim of isolating and identifying the causal agents, verifying their homology, comparing their morphology, testing their pathogenicity and formulating hypotheses regarding the factors responsible for their spread.

  Material and methods  

Study sites and their environmental features

Chestnut orchards were selected in October 2011 in three Italian regions: Boarda (Val di Susa, Turin, Piedmont), Montesenario (Mugello, Florence, Tuscany) and Crosano (Val d’Adige, Trento, Trentino-South Tyrol). The general environmental features of each stand are reported in Tab. 1.

Tab. 1 - Main environmental features of the study sites.

Site Boarda Montesenario Crosano
Elevation (m a.s.l.) 565 650 550
Exposure North North West North East
Morphology Terrace Terrace Slope
Slope 0% 5% 15%
Substrate Alluvial Sandstone Turbidite
Management cultivated Semi-cultivated Semi-cultivated
Irrigation Twice (July, August) absent absent
Geographic
coordinates
45.120369 N
7.187719 E
43.891551 N
11.330627 E
45.827764 N
10.975599 E

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Monthly mean temperatures and accumulated precipitation for 2011 were obtained from the meteorological stations closest to each of the study sites: Castel Borello (630 m a.s.l. - Società Meteorologica Italiana network), Borgo San Lorenzo (193 m a.s.l. - LaMMA network), and Besagno (382 m a.s.l. - FEM agro meteorological network). Only raw, non-validated, non-gap-filled meteorological data series were used. For Besagno, monthly mean temperatures and accumulated precipitation recorded during the vegetative period (April-September) were extracted from data for the whole period 2001-2011. These monthly values were compared with the average of the 10 years data series.

Sample collection and laboratory testing

Three chestnut trees were randomly selected in each of the orchards investigated. Forty nuts were collected from burrs still attached to the branches of each tree and sixty nuts were collected from the ground under the same trees. Burrs were examined for perithecia presence. Fruit samples were packaged separately in paper bags and immediately transferred to the laboratory for assays. Each nut was dissected and examined: fruits showing brown rot were separated from nuts affected by black rot and selected for isolation. A further 10 nuts were collected from ground in each area, stored in field conditions and evaluated for the presence of fruiting bodies.

Ten shoots were randomly collected from the crown of each tree, placed in plastic bags and stored at 4 °C for laboratory assay.

Fungal isolation and identification

(A) From nuts

Tissue from the initial decaying endosperm and from mummified fruits were surface- sterilized for 1 min in 70% ethanol, 5 min in 1.25% sodium hypochlorite and 30 sec in 70% ethanol. They were then rinsed twice in sterile, distilled water and blotted on dry sterile filter paper. Using a sterile scalpel, fragments of infected tissue were plated onto Potato Dextrose Agar (Difco, USA) containing biotin (1mg/l) and methionine (100 mg/l - PDAmb) and incubated in Petri dishes in the dark at 25 ± 1° C for seven days.

Fungal cultures were sub-cultured onto PDAmb in the dark at 25°C.

Morphological observation of colonies was carried out with an SMZ1000 stereomicroscope (Nikon, USA), while microscopic features, such as size, shape, color and arrangement of conidia, were observed with an Eclipse 80i microscope (Nikon). Measurements of 50 pycnidia and 50 conidia of one strain from each area plus 50 conidia collected from fructifications on nuts were made from digital sight images (DS-L2 imaging controller, Nikon, USA).

Brown rot mycelium was placed in 10 ml of sterilized tap water and shaken. One ml of conidial suspension (2 x 103 conidia ml-1) was diluted 1:5 with sterile tap water and plated on Petri dishes containing PDAmb substrate. Individual germinated conidia were collected under sterile conditions with a micro-needle using a stereomicroscope then transferred to plates and incubated under the conditions reported above. Thirty six individual conidial strains from each area were examined for morphological characteristics.

(B) From shoots

An 8-10 cm section was cut from each shoot of the current years’ and the two-year growth. Each sample was surface disinfested for 10 sec in 95% ethanol followed by 4 min in 2% NaOCl solution with 2 drops of Tween 80 l-1 ([38]). Ten fragments were cut from various positions on the bark tissue of each sample and placed on potato dextrose agar (PDA, Oxoid) in Petri dishes, five in each dish.

Isolations were incubated at 25 ± 1 °C for 7 days in the dark, after which the growing fungi were identified by their cultural characteristics. The number of fragments colonized by each type of culture was linked with the original sample and plot.

DNA analysis

DNA assays were carried out using cultures from individual monoconidial strains randomly selected from each area, two from Crosano and one from each of the other sites. Genomic DNA was extracted from approximately 50 mg of mycelia scraped from the surface of a 7-10 days culture growing on PDAmb. DNA was also extracted directly from initial decaying, brown tissue and chalky tissues in symptomatic nuts from Crosano. A total of seven strains were so assayed.

DNA was extracted using the NucleoSpin1 Plant Kit according to the manufacturer’s instructions (Macherey-Nagel, Düren, Germany). Internal transcribed spacer regions 1 and 2, including the 5.8S rDNA, were amplified and sequenced using the primers ITS5 and ITS4 ([48]). Gene fragments were amplified in 25 μl reactions on a GeneAmp 9700 thermal cycler (Applied Biosystems, Foster City, CA) under the following reaction conditions: 12.5 μl of GoTaq Green Master Mix (supplied in 2X Green GoTaq® Reaction Buffer pH 8.5, 400μM of each dNTPs and 3mM MgCl2 - Promega, USA), 0.40 μM of each primer, 10 ng of DNA template and 9.5 μl of nuclease free water. The thermal cycler programme was: 2 min at 95° C followed by 30 cycles of 30 sec at 95° C, 30 sec at 55 °C, and 1 min at 72 °C, with a final extension period of 10 min at 72 °C. Amplification products were separated by electrophoresis on 1% agarose gel at 100V for 30 minutes in TBE buffer (Tris-borate EDTA). The gel was stained with SyberSafe (Applied Biosystems, California, USA) and visualized on a UV transilluminator (Biorad) to asses PCR amplification.

PCR products were purified using Exo-SAP (Euroclone S.p.A., Italy) following the manufacturer’s instructions. Amplified products were sequenced with the Big Dye terminator v3.1 cycle sequencing kit (Applied Biosystems, Foster City, CA, USA) on an Applied Biosystems 3130xl Genetic Analyzer. BLASTN comparison of the amplicon sequences was carried out using the NCBI database to confirm the identity of the strains. Raw sequences were edited using Sequencer version 4.5 for Windows (Gene Codes Corporation, Ann Arbor, MI, USA) and deposited in the GenBank.

Nucleotide sequences were aligned with other fungal sequences (Gnomoniopsis spp., Phomopsis spp. and Phoma spp.) from NCBI using the Mega 4.1 software (⇒ http:/­/­www.­megasoftware.­net). A distance matrix was generated and an evolutionary tree for the datasets was inferred by the neighbor-joining method. The stability of relationships was assessed by bootstrap analysis of the neighbor-joining data based on 1000 replicates.

Artificial inoculation on nuts

Some 105 asymptomatic nuts were collected in a chestnut orchard near Trento (Lisignago), where no brown rot symptoms have been recorded until now. A small sample (15 nuts) was randomly chosen and dissected to confirm healthy status. Sixty of the remaining nuts were surface-sterilized for 1 min in 70% ethanol, 5 min in 1.25% sodium hypochlorite, 30 sec in 70% ethanol and rinsed in sterilized tap water. After this treatment, the fruits were artificially infected with each of the monoconidial strains selected for the DNA assay. An artificial wound 0.5 cm deep was made in the pericarp at the apical part of the fruit using a sterilized scalpel, as reported by Voglino & Bongini ([44]). A fragment of mycelium collected from a ten-day-old culture was placed in the wound, which was then covered with masking tape; the nuts were then stored in Petri dishes (25 cm in diameter). Fifteen replicates were run for each strain, another fifteen were wounded but not inoculated to serve as controls. The remaining fifteen unsterilized nuts were wounded as additional controls. All the treated and untreated nuts were stored at 25 °C in the dark. After twenty days all replicates were examined for disease and re-isolations were carried out from the symptomatic nuts on plates containing PDAmb.

Statistical analysis

The statistical analysis concerned the symptoms presence and isolations from nuts and shoots. For each symptom detected on nuts, considering the mean value of the three sampled trees, the three sites were compared using the Chi-square (χ2) test for 2-way tables (coupling the sites two by two). The same analysis was used for fungal isolation from bark tissue of shoots. χ2 values were compared with critical χ2 value at significance level α=0.05 and 1 degree of freedom.

  Results 

Study sites and environmental features

The three sites, located at similar altitudes, vary in exposure and morphology (Tab. 1). They are characterized by three different, but mainly acidic, geological substrates (Alluvial, Sandstone and Turbidite). Different management systems are in operation in the three orchards: Boarda is regularly cultivated (pruned and mowed) and irrigated twice during the summer, while Montesenario and Crosano are partially cultivated: mowing and harvesting are the only agricultural practices employed.

During 2011, high temperatures (over 20 °C) were recorded for August and September, while in the same months rainfall was less than 100 millimeters at all three stations (Fig. 1). In Besagno, August and September 2011 monthly mean temperatures were higher (1.3 and 2.7 °C, respectively) than the average of 10 years series for the same months (data not showed), while precipitations were lower of about 20 mm with respect to the same months and about 50 mm less for April and May. June and July were wetter with precipitations higher by 50 mm more than the 10 years series average for the same months (data not shown).

Fig. 1 - Monthly precipitation and mean temperatures recorded during 2011 at the three meteorological stations closest to the study sites.

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D. kuriphilus galls were observed in abundance at all the study sites.

Sample collection and description of symptoms

Significant differences were found between healthy fruits collected from the ground at Crosano and those collected at the other two sites (Tab. 2). The percentages of nuts displaying insect damage collected from the trees and from the ground was recorded for each of the study sites (range 15-23%). C. splendana and C. fagiglandana larvae were detected in the affected nuts and fungal rot associated with larval galleries was also observed.

Tab. 2 - Percentages of damaged nuts found in the samples collected from the three different chestnut orchards. Chi-squared test 2-way tables was performed. Critical χ2 value was at α=0.05 and df = 1. (*): values which differ in a significant way.

Symptoms Nuts from the ground Nuts from burrs
Boarda Montesenario Crosano Boarda Montesenario Crosano
No Symptoms (%) 62 65 32 81 72 56
Black rot (%) 8 7 3 2 1 0
Brown rot (%) 11 8 49* 2 4 24*
Insect damage (%) 19 20 16 15 23 20

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The main symptoms recorded in the remaining rotten nuts of the samples were of black rot (Fig. 2a) and brown rot (Fig. 2b).

Fig. 2 - (a) Nut completely destroyed by black rot due to Sclerotinia pseudotuberosa: it generally starts in the torch, producing grey coloration on the endosperm that rapidly turns blackish with evidence of black mycelium in the rotten tissue. (b) Nut affected by brown rot: the fungus initially causes light brown coloration on the margin of the endosperm, followed by loss of tissue consistency as it whitens and hardens, resulting in a chalky appearance. (c) Black pycnidia from brown rot tissue erupting below the episperm. (d) Culture of Gnomoniopsis sp.: colony on PDAmb. (e) Conidia obtained from stroma or pycnidia in cultures and from pycnidia on nuts. (f) Pycnidia of Gnomoniopsis sp. on Asian chestnut wasp gall.

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Initial and final symptoms coexisted in most of the nuts and, in a few cases, black and brown rot were observed together. Both rots were present in the nuts collected from the ground and in those still on the trees, although the extent of damage was greater in the nuts on the ground: black rot affected 8% of nuts gathered from the ground and 2% of nuts on the trees in the Boarda area, while the figures for Montesenario were 7% and 1%, respectively, and for Crosano 3% and 0%, without significant differences among sites (Tab. 2).

Brown rot was widespread in the Crosano area, where 49% of the nuts from the ground and 24% of the nuts from the trees showed symptoms. In this stand, the disease was significantly more present than in the other two sites either in nuts taken from the ground (vs. Boarda: χ2=19.21, p<0.05; vs. Montesenario: χ2=23.64, p<0.05) or from the burrs (χ2=6.27, p<0.05). The brown rot was also present in the other areas without significant differences: in Boarda 11% of the nuts from the ground and 2% of the nuts from the trees were affected, while in Montesenario the figures were 8% and 4%, respectively. In neither of these areas the disease was observed in previous years. No differences between the three sites were observed for insect damage.

Storage of the nuts, whether controls or producing fruiting bodies in natural conditions, exacerbated the brown rot as all the fruits displayed chalky tissue after three months. An abundance of pycnidia, first brownish-grey then blackish, appeared on the surface of the endosperm below the episperm (Fig. 2c). These fructifications were also observed in the invaginations and inside the endosperm where holes and cavities in the rotten tissue were detected. Conidia collected from these pycnidia were analogous to those obtained from the cultures (Tab. 3). No perithecia were observed on collected burrs and on infected nuts.

Tab. 3 - Comparison of conidiomata, conidia and cultural characteristics of fungi associated with brown rot obtained in this study compared with other findings reported in the literature. All studies cited reported the fungus on Castanea sativa. (n.r.): not reported.

Strains Perithecia
(μm)
Conidiomata
(μm)
Conidia
(μm)
Cultural morphology Symptoms
Gnomoniopsis sp.
(this study)
- 200 x 158 5.1-8.9 x
1.9-3.9
Light brown mycelium. Orange masses of conidiomata in concentric rings Brown rot,
endophytic on shoots
Phoma endogena
([37])
n.r. n.r. 6-8 x 2-3 Not reported Brown rot
Phoma endogena
([44])
- 200 x 160 6-7.5 x 2.4 Light brown mycelium. Orange masses of conidiomata in concentric rings Brown rot
Phoma endogena
([24])
- n.r. 8.1 x 2.4 White mycelium in concentric rings Brown rot, necrosis on shoots and leaves
Gnomoniopsis sp.
([17])
- n.r. 5.5-8.0 x
2.0-3.0
Light brown mycelium. Orange conidiomata in concentric rings Colonisation of D. kuriphilus galls
Gnomoniopsis castanea
([43])
- 244-268 x
146-190
4.9-7.3 x
2.4-3.7
Greyish brown mycelium with concentric rings of conidial stroma Brown rot,
endophytic on shoots
Gnomoniopsis smithogilvyi
([31])
238-242 - 6.5-9.5 x
2.0-4.0
Greyish brown mycelium with concentric rings of conidial stroma Brown rot,
endophytic on shoots

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Fungal isolation and identification

Cultures of greyish-black mycelia were isolated from black rot tissue and identified as the species Sclerotinia pseudotuberosa (syn. Ciboria batschiana, anamorph Rhacodiella castaneae) according to the morphological diagnostic criteria described by Ellis & Ellis ([11]).

Colonies with light brown mycelium were isolated from initial brown tissue and white, chalky tissue. Orange masses of conidial growth appeared in concentric rings on the surface of the cultures (Fig. 2d). On older colonies, blackish, ellipsoid pycnidia (158-200 μm) also produced conidia, which were generally ovoid, oval or oblong (5.15-8.91 µm x 1.90-3.96 µm - Fig. 2e). Based on the above characteristics the fungus was identified as Gnomoniopsis sp. (Tab. 3). Homogeneous morphological characteristics were found in all the monoconidial strains from all the study sites. Observed differences in size between conidia produced on chestnut fruits and those produced on nutritive media were non-significant.

High percentages of positive isolation were obtained from the bark tissue of both one-year and two-years-old shoots at each site (Tab. 4). Most of the colonies displayed the same characteristics as the fungus obtained from isolations from brown rot nuts. As for 1-year-old shoots, Crosano recorded the highest presence of Gnomoniopsis with respect to the Boarda and Montesenario (χ2= 21.9 and 27.4, respectively; p<0.05). Colonies of the brown rot agent were found on 70% of the fragments, on average. Boarda (33%) and Montesenario (48%) showed similar values as for one-year-old shoots, while they differed for 2-years-old shoots (χ2=4.67; p<0.05). Sporadic isolates of Cryphonectria parasitica were obtained, though no differences in frequencies were observed among sites. Crosano recorded also a presence of other fungi higher than Montesenario in one-year and two-years-old shoots (χ2=13.21 and 8.99, respectively; p<0.05). Tab. 3 reports a comparison of the morphological characteristics of these isolates of Gnomoniopsis sp. with those of fungi associated with the same symptoms reported by other authors ([37], [44], [24], [17], [43], [31]).

Tab. 4 - Mean percentage of fungi isolations from bark tissue of healthy shoots (one- and two-years old) of chestnut plants. The Chi-squared test for 2 way table was performed (presence/no presence for each isolate and coupled sites). Critical χ2 value at α=0.05 and df=1. (*): values which differ in a significant way.

Shoots Species Crosano Montesenario Boarda
1 year old Gnomoniopsis sp. 70* 33 37
Cryphonectria parasitica 0 1 0
other fungi 21* 4 9
Sterile fragments 9 61 55
2 years old Gnomoniopsis sp. 71* 48* 33
Cryphonectria parasitica 4 1 3
other fungi 17* 4 9
Sterile fragments 9 47 55

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DNA analysis

Morphological identification of fungal isolates was confirmed with molecular data obtained from DNA amplification. Four ITS sequences obtained from the DNA of fungal cultures and three sequences obtained directly from nut tissue were analyzed. A Megablast search in NCBI revealed the above fungal specimens having the highest similarity with the Gnomoniopsis sp. strain M6EmB (JN793536.1), with identity rates in the range of 99-100% (Tab. 5).

Tab. 5 - Database matches for sequences generated from ITS 5 and ITS 4 PCR products, derived from tissue showing symptoms of brown rot and mycelia of monoconidial cultures.

Isolate DNA origin Description Max ident.
(%)
Gm_TN1 Trentino mycelium Gnomoniopsis sp. M6EmB (JN793536.1) 99
Gm_TO Piedmont mycelium Gnomoniopsis sp. M6EmB (JN793536.1) 100
Gm_FI Tuscany mycelium Gnomoniopsis sp. M6EmB (JN793536.1) 99
Gm_TN2 Trentino mycelium Gnomoniopsis sp. M6EmB (JN793536.1) 99
Gn_TN3 Chalky tissue Gnomoniopsis sp. M6EmB (JN793536.1) 99
Gn_TN4 Brown tissue Gnomoniopsis sp. M6EmB (JN793536.1) 99
Gn_TN5 Initial brown tissue Gnomoniopsis sp. M6EmB (JN793536.1) 99

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Phylogenetic analysis of Gnomoniopsis spp., Phomopsis spp. and Phoma spp. revealed their classification in three distinct groups (Fig. 3), and a very close relationship between the Gnomoniopsis sp. strains from this study and those found in GenBank derived from Dryocosmus galls (Viterbo) and chestnut rot in Italy (Torino - Gnomoniopsis castanea), Australia (Gnomoniopsis smithogilvyi) and New Zealand, as well as with strains from India whose host was not specified in the database (Fig. 3). The chestnut Gnomoniopsis sequences seem quite different from other Gnomoniopsis strains detected in the USA on other plant species. The Phomopsis castanea sequence is completely different from Gnomoniopsis ones; this strain derived from Castanea mollissima in China, but no other information are recorded.

Fig. 3 - Dendrogram showing the similarities between amplificates from mycelium isolates and nut tissue samples (boldface) and sequences in the NCBI database created by the CLUSTALW software.

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Artificial inoculation of nuts

All fifteen nuts assayed to test their healthiness were found to be uncontaminated by moulds.

The Gnomoniopsis isolates tested engendered symptoms of brown rot and were detected in most (61 to 71%) of the artificially infected nuts. No differences between the strains were evident (Tab. 6). The disinfected and wounded controls did not show any symptoms, while only two (13%) of the wounded but non-disinfected controls showed initial symptoms of colonization by Penicillium sp.

Tab. 6 - Results of the artificial inoculation tests. (*): 13% (2 nuts) affected by Penicillium spp.

Strain % nuts affected
by brown rot
%
asymptomatic
Gm_TN1 71 29
Gm_TN2 72 28
Gm_FI 62 38
Gm_TO 61 39
Control (disinfected and wounded) 0 100
Control (not disinfected, wounded) 0 87*

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  Discussion and conclusions 

A high degree of damage was found in all three orchards sampled and both black rot and brown rot fungi were common, especially in the Crosano orchard where more than half of the crop appeared to be affected by mould fungi. Insect damage was also severe, confirming its destructiveness in nut production.

Sclerotinia pseudotuberosa is known to be a ubiquitous endophyte capable of direct nuts colonization, starting with infection of the flowers ([42]). Warm, dry weather during the harvest period, as recorded in 2011, may have restricted the presence of the fungus in the nuts sampled. Indeed, several authors consider these conditions to be the main factors constraining the spread of black rot ([34], [10], [24]). Nonetheless, it is worth noting that black rot was present in all the study areas and could pose a serious problem for nut storage in the absence of water-curing treatments ([18]).

The unusual spread of brown rot, the high incidence of damage caused by this disease and the extent of the damage found in Crosano justifies growers’ worries about this disease, which has been highly destructive in other parts of Piedmont and Tuscany ([43], Poli, personal comm.). The presence of brown rot in fruits still in the burr exacerbates the already harmful impact of this disease and reduces the quality and quantity of chestnuts with consequences for the economic viability of cultivation.

Gnomoniopsis sp. was found to be the causal agent of brown rot in all three areas. In addition to genetic analyses, culture morphology and the shapes and sizes of conidia also confirm homology of the isolated strains with those recently found in association with D. kuriphilus galls in the Viterbo area (Monti Cimini - [17]). We were also able to confirm a complete homology with the newly described Gnomoniopsis castanea ([43]) and Gnomoniopsis smithogilvyi ([31], [32]). As suggested by Vannini et al. ([41]) and Visentin et al. ([43]), evidence by isolation from bark support a massive presence of this fungus as endophytic in one- and two-year-old shoots. This behavior could explain its ability to colonize gall tissue and to infect nuts still in burrs, maybe in bud burst. It could also explain its sudden appearance in various chestnut-growing areas of Italy, because probably already present on trees. Nevertheless, this fungus, like S. pseudotuberosa, was not reported in previous investigations on endophytism in chestnut shoots carried out in Switzerland ([3]). Other fungi belonging to the Gnomoniopsis genus were also described as endophytic on Fagacae ([45]). It is worth noting that isolation of Gnomoniopsis was not related to bark alteration (cankers or necrosis) and that no fructification was observed on bark tissue in the present study, while pycnidia were found on galls instead. The common presence of this fungus on chestnut tissue suggests a possible role in checking gall wasp populations by colonizing the gall tissue and perhaps the insect inside chambers ([41]), but its pathogenicity on fruits is a formidable constraint for its potential use as a bio-control agent.

According to the owner of the Crosano orchard, brown rot has been present since 2003, although its presence has increased in the last three years. Its emergence does not appear to be related to the appearance of D. kuriphilus infestations in Trentino, which was first recorded in the province in 2007 and far away from the stand examined ([29]). The recent finding (January 2013) of Gnomoniopsis pycnidia on galls which remained overwintering on trees (Fig. 2f - Maresi G, personal comm.) calls for a more detailed investigation on the possible role of D. kuriphilus galls in the spread of the brown rot fungus.

Meteorological records report a warm, dry period in all the study areas during the 2011 vegetative season, but in the area least affected (Boarda) irrigation helped the trees. Stress and drought periods have been common in the Crosano area since 2003. Plant stress brought about by drought and gall wasp attacks may have favored brown rot spread in central and northern Italy. Afflicted and suffering chestnut trees are likely to be highly susceptible to infection by endophytes or latent pathogens such as Gnomoniopsis sp., as they have been to chestnut blight ([39]). In a context of climate change, new interesting perspectives arise for the concept of parasitism: asymptomatic fungi may become virulent and produce disease symptoms under certain environmental conditions ([6], [35], [25], [16]). It is worth noting that temperatures around 27 °C are considered optimal for the growth of Phoma endogena, the causal agent of brown rot, according to Ridé & Gudin ([24]).

Gnomoniopsis sp. was isolated from initial brown decaying tissue, white chalky tissue and blackish fruiting bodies on decayed endosperm. There is a close correspondence between these symptoms and those of Phoma endogena, first described by Spegazzini ([37]) on nuts in the Veneto region (northern Italy). Voglino & Bongini ([44]) gave an accurate account of the degradation of infected nuts collected in Piedmont, and the symptoms and pycnidia described, as well as the photographs, closely match those of Gnomoniopsis sp. Servazzi ([30]) used the term “mummification” for the same phenomenon observed on nuts from the same area (Piedmont), while Ciferri ([8]) reported that Servazzi’s description corresponded with the symptoms he observed on nuts collected near Cuneo (Piedmont). He proposed the new name Phomopsis endogena based on the presence of a very few Phomopsis type β conidia and suggested that P. endogena may be identical with Phomopsis viterbensis from the Viterbo area described by Camici ([7]). Moreover, working with Voglino & Bongini’s ([44]) original strains, he confirmed homology in morphology between Phoma and Phomopsis endogena. Ciferri also suggested that this fungus was already present in the nut during fructification and therefore in burrs. Remarkably, all these reports refer to the areas where the main attacks of Gnomoniopsis sp. are currently being observed. Ridé & Gudin ([24]) introduced the term “brown rot” (pourriture brune) and revived the name Phoma endogena for the absence of type β conidia: their descriptions of the mycelium and symptoms closely match those reported by the aforementioned authors and those described in this paper. They also hypothesized that infection occurred at early fructification stages, that P. endogena was possibly endophytic, and that there was a relationship between the action of the fungus and warm temperature and dry conditions. Breisch ([5]) and Pratella ([23]) showed clear pictures of P. endogena attacks in their papers, which perfectly match the symptoms observed in the present study. The same rot disease has also been ascribed to Gnomonia pascoe in New Zealand ([36]). Ho (pers. comm.) recently pointed out the genetic correspondence between P. castanea, P. endogena and Gnomoniopsis sp. in New Zealand, while in Australia Shuttleworth et al. ([31], [32]) put forward the name Gnomoniopsis smithogilvyi instead of G. pascoae for the agent of brown rot damage. Eventually, the same fungus was described in Piedmont as Gnomoniopsis castanea ([43]). Unfortunately, no Phoma or Phomopsis endogena cultures or DNA sequences are recovered for comparison with Gnomoniopsis sp.

Montealegre & Gonzalez ([19]) in Chile and Washington et al. ([47], [46]) in Australia both indicated Phomopsis castanea as agents of brown rot in Castanea sativa orchards, though they did not describe or record type β conidia. Phomopsis castanea was instead recovered from cankers on small branches and shoots of European chestnut but not on nuts ([26], [27], [28], [22], [20], [1]). Recently, a Phomopsis castanea mollissima was described on leaves but not on fruits of Castanea mollissima in China ([33]). On this basis, Smith & Agri ([36]) clearly distinguished between Phomopsis or Diaporthe castanea found on chestnut older branches and Gnomonia pascoe agent of brown rot, then described as Gnomoniopsis by Shuttleworth et al. ([31]).

In conclusion, Phoma endogena, Phomopsis endogena, Gnomonia pascoe, Gnomoniopsis castanea, Gnomoniopsis smithogilvyi and Gnomoniopsis sp. have very similar morphological characteristics and pathogenic behavior, in that they have similar-sized pycnidia and conidia and are able to produce the same array of symptoms in chestnut nuts, being also all endophytic in bark tissues. Therefore, the hypothesis that they could be the same fungus is very plausible. Anyway, further studies on the taxonomy and genetics of these fungi are required, given that DNA analyses clearly separate the Phoma, Phomopsis and Gnomoniopsis groups. Nonetheless, Gnomoniopsis sp. is the agent involved in the current epidemic of brown rot, and recovered on D. kuriphilus galls in Italy, like the brown rot pathogen recorded in Australia. In the light of these findings, further researches are desirable to find new control strategies aimed to save production in the most affected areas. The need is urgent as there is a risk that a combination of various factors, such as the resurgence of blight due to climate stress, the expansion of the Asian chestnut gall wasp and crop destruction by fungi or insects, could set off a general decline in chestnut trees and orchards or, even worse, in the entire chestnut production.

  Acknowledgements 

We would like to thank Giovanni Falchero, Paolo Miorelli, Luciano Massetti and Francesca Ugolini for technical assistance in the field and data processing.

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Authors’ Affiliation

(1)
G Maresi
FEM-IASMA - Centre for Technology Transfer, v. E. Mach 1, I-38010 San Michele all’Adige (TN - Italy)
(2)
CM Oliveira Longa
FEM-IASMA - Research and Innovation Centre, Sustainable Agro-Ecosystems and Bioresources Department, v. E. Mach 1, I-38010 San Michele all’Adige (TN - Italy)
(3)
T Turchetti
Institute of Plant Protection (IPP-CNR), v. Madonna del Piano 10, I-50019 Sesto Fiorentino (FI - Italy)

Corresponding author

Citation

Maresi G, Oliveira Longa CM, Turchetti T (2013). Brown rot on nuts of Castanea sativa Mill: an emerging disease and its causal agent. iForest 6: 294-301. - doi: 10.3832/ifor0952-006

Academic Editor

Alberto Santini

Paper history

Received: Jan 21, 2013
Accepted: Apr 19, 2013

First online: Jul 16, 2013
Publication Date: Oct 01, 2013
Publication Time: 2.93 months

© SISEF - The Italian Society of Silviculture and Forest Ecology 2013

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