Abstract
A botryosphaeriaceous taxon causing fruit peduncle and pedicel discolouration was found infecting grapevines in Hubei and Jiangsu Provinces in China. Morphological and phylogenetic analyses showed the taxon to be Lasiodiplodia pseudotheobromae. Pathogenicity testing and Koch’s postulates proved that Lasiodiplodia pseudotheobromae caused fruit peduncle and pedicel discolouration on grape fruit clusters. This is the first report of this fungus causing grapevine fruit peduncle and pedicel discolouration worldwide.
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Grapes have been grown in China for more than 2000 years and grape production has increased rapidly, especially since the 1980’s (Li 2001). Grapevine trunk diseases cause great economic losses in the wine and grape industries across the world (Úrbez-Torres 2011). Botryosphaeriaceous pathogens associated with grapevine trunk diseases cause severe and economically significant symptoms (Crous et al. 2006; Úrbez-Torres 2011; Yan et al. 2013). The genera Botryosphaeria, Diplodia, Lasiodiplodia and Neofusicoccum were reported to be the prominent genera of Botryosphaeriaceae associated with grapevine infections (Luque et al. 2009; van Niekerk et al. 2006; Úrbez-Torres 2011). Presently 25 Botryosphaeriaceae species are known from grapevine worldwide (Úrbez-Torres 2011; Linaldeddu et al. 2014; Dissanayake et al., First report of Neofusicoccum mangiferae associated with grapevine dieback in China (unpublished)). Morphological and multi-gene phylogenetic analyses confirmed Botryosphaeria dothidea, Diplodia seriata, Lasiodiplodia theobromae and Neofusicoccum parvum were associated with different grapevine dieback symptoms in Chinese vineyards (Yan et al. 2013). Lasiodiplodia pseudotheobromae is reported for the first time on grapevine in Brazil as a grapevine trunk pathogen (Correia et al. 2013). The symptoms caused by Botryosphaeriaceae on grapevines are significantly different between countries and vary depending on the cultivars. The most serious symptom reported in Chinese grapevines are ‘cluster and fruit dropping’ which differs to the major symptoms described in other countries (Yan et al. 2013).
In June–August 2013, the disease was observed on grape clusters (E–L33) in Jiangsu and Hubei Provinces in China. The symptoms appeared on fruit peduncles and pedicels in grape clusters as small, brown necrotic lesions which expanded and later became dry and dead (Fig. 1). Symptomatic grape clusters were collected; the tissues were cut into 5 mm pieces from the margins of healthy and infected tissues and surface-sterilized by immersion in 2 % NaOCl for 1 min. The cuttings were rinsed three times in sterile distilled water, dried and placed on potato dextrose agar (PDA) medium and incubated at 28 °C for 7 days. Isolates developed from the diseased tissues were sub-cultured on PDA medium and purified via single spore isolation. Representative cultures were deposited at the Mae Fah Luang University culture collection (MFLUCC), Thailand (Table 1).
Identification of the fungus was based on both morphological characteristics and molecular methods. Conidiomata obtained from the culture plates were mounted in microscopic slides and the dimensions of 40 conidia were measured with Nikon DS-RiI digital camera connected to a Nikon NIS-Elements F3.0 microscope.
The genomic DNA was extracted from pure cultures grown on PDA following the CTAB method of Doyle and Doyle (1987). DNA amplification was performed by polymerase chain reaction (PCR). Primer pairs ITS1 and ITS5 (White et al. 1990) were used to amplify the internal transcribed spacers. Primers EF1–728F and EF1–986R (Carbone and Kohn 1999) and Bt2a and Bt2b (Glass and Donaldson 1995) were used to amplify and sequence part of the translation elongation factor 1-alpha (EF1-α) gene and part of the β-tubulin gene respectively. Sequences were aligned with those retrieved from GenBank (Table 1) using MAFFT v. 6.0 (Katoh and Toh 2010) and manually adjusted when necessary. Maximum parsimony analysis (MP) was performed with PAUP* (Phylogenetic Analysis Using Parsimony) v. 4.0b10 (Swofford 2003) using the heuristic search option with 1000 random stepwise addition. The nucleotide substitution models were determined individually for each gene region using MrModelTest v. 2.3 (Nylander 2004). A Bayesian analysis was performed using MrBayes v. 3.1.2 (Ronquist and Huelsenbeck 2003). Sequences generated in this study are deposited in GenBank (Table 1). Resulting alignment and the tree were deposited in TreeBASE (http://www.treebase.org/) as accession number S16881.
Pathogenicity was assessed for grape fruit clusters (E–L36) cv. Niunai. Grape clusters were surface sterilized with 1 % NaOCl and washed three times in sterilized water. Six peduncles and six pedicels were punctured with a sterile needle. Mycelial plugs (3–5 mm2) taken from the margin of an actively growing colony on PDA (isolate MFLUCC 14-1192) was placed on the wounded peduncles and pedicels. Sterile PDA plugs were placed on punctured peduncles and pedicels as controls. Wounds were sealed and wrapped with parafilm (BEMIS, USA). Inoculated grape clusters were maintained at 28 °C and 70 % RH under 12 h light/12 h dark system for 5 days.
Colonies on PDA were initially grey-white and became dark grey-black when aged with a sporulation after 15 days. Conidia were 25–30 × 10–15 μm (n = 40), hyaline, aseptate, sub-ovoid to ellipsoid with broadly rounded apices and later became dark brown, 1-septate and thick-walled (Fig. 2). Conidial morphology and cultural features of the isolates are in close agreement with the morphological description of L. pseudotheobromae (Alves et al. 2008).
Amplicons of the ITS, EF1-α and β-tubulin regions have approximately 0.5, 0.3, and 0.4 kbp, respectively. The combined dataset of ITS, EF1-α and β-tubulin consisted of 15 taxa, which comprised the four L. pseudotheobromae isolates obtained in this study and 11 additional isolates (Hyde et al. 2014) including the outgroup Diplodia mutila. The combined dataset comprised 1180 characters after the uneven ends were truncated. Of these characters, 1034 were constant, 111 were parsimony uninformative and 35 were parsimony informative. A heuristic search revealed most parsimonious trees (Fig. 3; tree length = 176 steps, CI = 0.898, RI = 0.822, RC = 0.738 and HI = 102). Maximum-parsimony and Bayesian inference produced trees with nearly identical topologies (Bayesian tree not shown). Isolates obtained in this study clustered together in a well-supported clade (bootstrap value = 100 %; posterior probability = 1.0) with the ex-type of L. pseudotheobromae (CBS 116459) thus confirming the identification of the studied isolates.
Disease symptoms developed on the inoculated fruit peduncles and pedicels within 24 h after inoculation. At the end of the third day, grey-white mycelia were observed on affected areas (Fig. 4). The pathogen was re-isolated from the lesions on peduncles to confirm Koch’s postulates. No disease symptoms were observed on the control fruit clusters.
On the basis of morphological characteristics, pathogenicity testing on host plant, and molecular analysis, the fungus was identified as L. pseudotheobromae. This species was previously reported in China on Acacia confusa, Albizia falcataria, Eucalyptus sp., Mangifera sylvatica and Paulownia fortunei (Zhao et al. 2010). To our knowledge, this is the first report of Lasiodiplodia pseudotheobromae causing grapevine fruit peduncle and pedicel discolouration worldwide.
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The study is funded by CARS-30 and CXJJ201402.
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Asha J. Dissanayake and Wei Zhang contributed equally to this work.
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Dissanayake, A.J., Zhang, W., Mei, L. et al. Lasiodiplodia pseudotheobromae causes pedicel and peduncle discolouration of grapes in China. Australasian Plant Dis. Notes 10, 21 (2015). https://doi.org/10.1007/s13314-015-0170-5
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DOI: https://doi.org/10.1007/s13314-015-0170-5