Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China

Li, Hui; Peng, Bing-Yao; Xie, Jun-Ya; Bai, Yu-Qing; Li, De-Wei; Zhu, Li-Hua

doi:10.3390/jof10030230

Open AccessArticle

Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China

by

Hui Li

^1,2,

Bing-Yao Peng

^1,2,

Jun-Ya Xie

^1,2,

Yu-Qing Bai

^1,2,

De-Wei Li

³

and

Li-Hua Zhu

^1,2,*

¹

College of Forestry and Grassland, Nanjing Forestry University, Nanjing 210037, China

²

Co-Innovation Center for Sustainable Forestry in Southern China, Nanjing Forestry University, Nanjing 210037, China

³

The Connecticut Agricultural Experiment Station Valley Laboratory, Windsor, CT 06095, USA

^*

Author to whom correspondence should be addressed.

J. Fungi 2024, 10(3), 230; https://doi.org/10.3390/jof10030230

Submission received: 3 February 2024 / Revised: 3 March 2024 / Accepted: 19 March 2024 / Published: 21 March 2024

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Abstract

:

Pinus massoniana Lamb. is an important, common afforestation and timber tree species in China. Species of Pestalotiopsis are well-known pathogens of needle blight. In this study, the five representative strains were isolated from needle blight from needles of Pi. massoniana in Nanjing, Jiangsu, China. Based on multi-locus phylogenetic analyses of the three genomic loci (ITS, TEF1, and TUB2), in conjunction with morphological characteristics, a new species, namely Pestalotiopsis jiangsuensis sp. nov., was described and reported. Pathogenicity tests revealed that the five representative strains of the species described above were pathogenic to Pi. massoniana. The study revealed the diversity of pathogenic species of needle blight on Pi. massoniana. This is the first report of needle blight caused by P. jiangsuensis on Pi. massoniana in China and worldwide. This provides useful information for future research on management strategies of this disease.

Keywords:

multi-locus phylogeny; new species; pine

1. Introduction

Pinus massoniana Lamb. is the most widely distributed timber tree species with the largest afforestation area in China [1], which provides a large amount of timber, oleoresin [2], carbon storage [3], and ecological products [4], and also has potential biomedical properties [5]. However, Pi. massoniana was found dead at the top of needles in plantations in Nanjing, Jiangsu Province with a high incidence, which seriously threatened the economic and ecological value.

Many pathogens have been reported to damage Pi. massoniana in the world; for example, its forestry and pine forests were threatened by outbreaks of pine wilt disease (PWD) caused by Bursaphelenchus xylophilus (pinewood nematode; PWN) [6]. Damping-off and root rot disease caused by Fusarium oxysporum has been found in Pi. massoniana [7,8]. Pseudofusicoccum kimberleyense and Pse. violaceum can cause dead branch disease of Pi. massoniana [9]. Pestalotiopsis funerea affected the needles of young Pi. massoniana trees and caused them to gradually dry up and fall off [10]. In addition, insect–parasitic entomopathogenic fungi such as Penicillium citrinum, Purpurecillium lilacinum, and Fusarium spp. were also confirmed to be pathogenic to Pi. massoniana [11]. However, as an important economic tree species, the host–pathogen relationship of Pi. massoniana needs more studies, and additional pathogens may be found.

Pestalotiopsis species are widely distributed in the world as endophytes, plant pathogens, or saprobes [12,13,14,15,16,17], mainly in tropical and temperate regions and have a wide range of host plants [15,18,19]. Initially, the characteristics of conidia, such as color, size, and appendages, are the key to the identification of Pestalotiopsis and related genera [20,21]. Those taxonomic groups related to the genus Pestalotiopsis are also called pestalotioid fungi. Afterwards according to the relationship between conidial morphology and multi-locus phylogeny [14,19,22,23], Pestalotiopsis sensu lato was divided into three genera by Maharachchikumbura et al. (2014) [15]—Pestalotiopsis sensu stricto, Neopestalotiopsis, and Pseudopestalotiopsis. Three genera correspond to three types of conidia, conidia with light brown or olivaceous concolorous median cells (Pestalotiopsis sensu stricto), conidia with versicolorous median cells (Neopestalotiopsis), and conidia with dark-colored concolorous median cells (Pseudopestalotiopsis) [14,19,22,24]. Pestalotioid species identification remains a major challenge because of the conidia of overlap, and the classification is complex [22,25,26].

Needle blight caused by Pestalotiopsis is a common disease in young pine forests, and the disease is widely distributed and causes serious damage. For example, Pestalotiopsis funerea can infect Pinus tabulaeformis [27], Pi. taeda [28], Pi. massoniana [10], etc. and cause needle blight. Xu et al. (2017) [29] reported that the pathogen causing the needle blight of Pi. sylvestris was P. citrina. The disease began to occur in 1974 and became popular in 1980, and it has become the main coniferous disease of trees [30,31]. Needle blight not only reduced the stock of trees but even led to the death of trees, which greatly threatened forestry production [32,33,34].

In March 2023, the needles of Pi. massoniana with the characteristics of needle blight were collected in Nanjing, Jiangsu Province. The earlier identification of Pi. massoniana needle blight in a previous study was in a different geographical area [10]; thus, the main purpose of this study was to determine the pathogen of Pi. massoniana needle blight and its pathogenicity by Koch’s postulates.

2. Materials and Methods

2.1. Field Survey and Fungal Isolation

In March 2023, needle lesions were found on Pinus massoniana in Lishui District, Nanjing, Jiangsu, China. The entire planting area of the Pi. massoniana forest was about 1800 m². The symptoms of trees were visually observed and the needles with the symptoms were collected. Five symptomatic Pi. massoniana trees were randomly sampled. After macroscopic and microscopic observation of the collected pine needles, the pine needle fragments at the intermediate area of the diseased and healthy portions were cut off, and the surface was disinfected in 70% ethanol for 30 s, in 1% NaClO for 90 s, and then washed in sterile water for 90 s three times. Pine needle fragments were dried on sterile filter paper and incubated on potato dextrose agar (PDA) in the dark at 25 °C for 3 days. The hyphal tips of fungi emerging from tissue pieces were transferred to new PDA to obtain pure cultures. The isolates were obtained from needle blight samples of Pi. massoniana.

2.2. Morphological Identification

Colony morphology and pigment production on PDA was observed after 7 days at 25 °C with a 12/12 h light/dark cycle and inspected daily for fungal sporulation. Acervuli and conidial masses were observed under a Zeiss stereo microscope (SteRo Discovery v20, Oberkochen, Germany). The micromorphological characteristics of five isolates were observed by Zeiss Axio Imager A2m microscope (Carl Zeiss, Oberkochen, Germany), such as shape, color, septation, appendages, and size of conidia, conidiophores, and acervuli.

2.3. Genomic DNA Extraction, PCR, and Sequencing

Fungal genomic DNA of fungi cultured on PDA for 5 days was extracted by the cetyltrimethylammonium bromide (CTAB) method, and three distinct DNA regions were amplified by polymerase chain reactions (PCR). Three genomic loci, including the internal transcribed spacer (ITS), the partial translation elongation factor 1-alpha (TEF1), and partial β-tubulin (TUB2), were amplified with primers ITS5/ITS4 [35], EF1-728F/EF1-986R [36], and T1/Bt-2b [37,38], respectively. The protocols for amplification are shown in Table 1. Each 50 μL PCR mixture consisted of 25 μL of Premix TaqTM (Takara Biomedical Technology Company Limited, Beijing, China), 19 μL of dd H₂O, 2 μL of forwarding primer, 2 μL of reverse primer, and 2 μL of DNA template. PCR purification and sequencing were performed by Sangon Biotech (Shanghai) Co., Ltd. (Nanjing, China).

2.4. Phylogenetic Analyses

Sequences with similarity of the ITS sequences generated in the present study were searched with the BLAST program on GenBank (https://blast.ncbi.nlm.nih.gov/, accessed on 3 November 2023), and the reference sequences used in this study were obtained. Concatenated multi-locus data (ITS, TEF1, and TUB2) were used for phylogenetic analyses with maximum likelihood (ML) and Bayesian Inference (BI). Neopestalotiopsis protearum (CBS 114178) was designated as an outgroup. The DNA sequences were aligned with MAFFT ver. 7.313 [39] and adjusted with BioEdit ver. 7.0.9.0 [40]. Maximum likelihood (ML) analysis was conducted on the multi-locus alignments using IQtree ver. 1.6.8 [41] with the GTR + F + I + G4 replacement model and the bootstrap method with 1000 replications to assess clade stability. RA × ML bootstrap support values were set at ML ≥ 70. Bayesian inference was analyzed using MrBayes ver. 3.2.6 with the GTR + I + G + F model (2 parallel runs, 2,000,000 generations) according to Quaedvlieg et al. (2014) [42]. Bayesian posterior probability values were set at PP ≥ 0.90. The phylogenetic trees were created in Figtree ver. 1.4.4. (http://tree.bio.ed.ac.uk/software/figtree/, accessed on 2 December 2023).

2.5. Genealogical Concordance Phylogenetic Species Recognition Analyses

The phylogenetically related ambiguous species were analyzed using the Genealogical Concordance Phylogenetic Species Recognition (GCPSR) to determine the recombination level in closely related species by performing a pairwise homoplasy index (PHI) test according to the method described by Quaedvlieg et al. (2014) [42]. A PHI result below 0.05 (Φw < 0.05) indicated significant recombination in the dataset. The relationships between closely related species were visualized in splits graphs with the LogDet transformation and splits decomposition options.

2.6. Pathogenicity Test

In this study, 12 two-year-old healthy Pi. massoniana seedlings and the three isolates representing the highest isolation frequency of Pestalotiopsis species were selected to perform the pathogenicity tests: BM 1-1, BM 1-2, BM 1-3—Pestalotiopsis jiangsuensis sp. nov. The tested plants were taken from the GuDong Green Seedling Base in Hechi, Guangxi Province, China. Healthy needles of Pi. massoniana were injured with a sterile needle. One wound was made per pine needle and conidial suspension (10⁶ conidia·mL⁻¹) was sprayed on the wounds. Three plants were inoculated with each isolate, and the control was treated with sterile water. Inoculated seedlings and control seedlings were placed in a tent (1.5 × 1.2 × 1.5 m) with a humidifier (300 mL/h) to maintain RH 70%. The tent was placed in a greenhouse at 25 ± 2 °C and observed continuously for 10 days. All experiments were conducted three times.

3. Results

3.1. Disease Symptoms and Fungal Isolation

In March 2023, the incidence of needle blight of Pi. massoniana found in Nanjing, Jiangsu Province was ca. 60%, and the needle disease incidence of each Pi. massoniana was as high as 80%. The early symptom was a small yellow lesion at the needle tip, which extended from the needle tip downwards, and the lesion turned gray; a dark brown band encircled the needle at the junction with the healthy part (Figure 1A–C). Eventually the lesion area expanded until all the needles were necrotic. Ninety Pestalotiopsis strains were isolated and determined, based on the colony morphologies on PDA and ITS sequence blasting, with an isolation frequency of 90% (90/100). Five representative isolates (BM 1-1, BM 1-2, BM 1-3, BM 1-4, and BM 1-5) were selected for further study and deposited at the China Forestry Culture Collection Center (CFCC).

3.2. Phylogenetic Analyses

The concatenated sequence dataset of ITS, TEF1, and TUB2 included the five representative isolates, 120 taxa, and one outgroup taxon (Neopestalotiopsis protearum CBS 114178) with a total of 1637 base pairs (1-554 for the TEF1, 555-1163 for ITS, and 1164-1637 for TUB2) including gaps were obtained. The hosts, locations, and GenBank accession numbers of Pestalotiopsis species used for phylogenetic analyses in this study were shown in Table 2. The tree topology of the phylogenetic tree of ML and BI systems was congruent, and the bootstrap support values of RA × ML greater than 70% and the Bayesian posterior probabilities greater than 0.90 were denoted at nodes. In the phylogenetic analyses, five isolates formed a separate clade (ML/BI = 100/1), which was clustered into a big branch with four ex-type strains with a significant support (ML/BI = 98/0.92: Pestalotiopsis foliicola CFCC 54440, P. pinicola KUMCC 19-0183, P. suae CGMCC 3.23546, and P. rosea MFLUCC 12-0258. Based on the three-locus phylogenetic analyses and morphology, five strains (BM 1-1, BM 1-2, BM 1-3, BM 1-4, and BM 1-5) were identified as a new species of Pestalotiopsis (Figure 2).

Importantly, the PHI test of new species shows that no significant recombination (Φw = 0.071) events were observed between Pestalotiopsis sp. (undescribed taxon) and phylogenetically related species P. foliicola CFCC 54440, P. pinicola KUMCC 19-0183, P. suae CGMCC 3.23546, and P. rosea MFLUCC 12-0258 (Figure 3).

3.3. Taxonomy

Pestalotiopsis jiangsuensis Li-Hua Zhu, Hui Li, and D.W. Li, sp. nov. Figure 4

Index Fungorum No: IF 900494

Etymology: the epithet referring to the province where the holotype was collected.

Description: Sporadic black and gregarious conidiomata produced on PDA after 7 days under light at 25 °C, globose, semi-immersed, dark brown to black, up to 400 μm diam (Figure 4B); conidiophores indistinct and reduced to conidiogenous cells. Conidiogenous cells (4.5-) 7.0–12.8 (−15.3) × (2.4-) 3.3 –5.6 (−6.5) µm (11.4 ± 2.5 × 4.4 ± 0.9 µm, n = 30), hyaline, ampulliform or cylindrical, and sometimes slightly wide at the base (Figure 4C). Conidia phragmospores, (20.3-) 22.1–25.5 (−27.3) × (6.2-) 6.7–8.2 (−8.7) µm (23.4 ± 1.8 × 7.5 ± 0.5 µm, n = 30), fusoid, ellipsoid, straight to slightly curved, 4-septate (Figure 4D); basal cell hyaline, obconic, thin-walled, 3.5–5.9 μm long; three median cells (12.7-) 13.7–15.5 (−16.5) × (6.2-) 6.7–7.4 (−7.9) µm (14.2 ± 1.0 × 7.2 ± 0.5 µm, n = 30), doliiform, wall rugose, concolorous, brown, septa darker than the rest of the cell (second cell from the base 4.2–5.9 μm long; third cell 4.8–5.7 μm long; fourth cell 4.0–5.4 μm long); apical cell hyaline, smooth-walled, conic or trapezoid, tapering toward the apex, 2.6–4.4 μm long, with 1–4 tubular apical appendages (mostly 2 and very few 4), arising from the apical crest, unbranched, filiform, 8.7–23.4 μm long; basal appendage single, tubular, unbranched, centric, 1.4–6.3 μm long.

Culture characteristics: Colonies on PDA flat with sparse aerial mycelia on the surface after 7 d at 25 °C, edge undulate, pale honey-colored, and reverse pale brown in the center and pale luteous margin (Figure 4A).

Holotype: China, Jiangsu province, Nanjing city, Lishui district, Baima National Agricultural Science and Technology Park, 119°10′44″ N, 31°36′28″ E (DMS), isolated from needles of Pinus massoniana, 1 March 2023, Hui Li, holotype CFCC 59538. Holotype is a living specimen being maintained via lyophilization at the China Forestry Culture Collection Center (CFCC), Chinese Academy of Forestry, Beijing, China, and ex-type BM 1-1 is stored at Forest Pathology Laboratory, Nanjing Forestry University.

Habitat and host: On needles of Pinus massoniana with needle blight.

Known distribution: Nanjing, Jiangsu Province, China.

Additional specimens examined: China, Jiangsu province, Nanjing city, Lishui district, Baima National Agricultural Science and Technology Park, 119°10′44″ N, 31°36′28″ E (DMS), isolated from needles of Pinus massoniana, 1 March 2023, Hui Li, cultures: CFCC 59539 (=BM 1-2), CFCC 59540 (=BM 1-3), CFCC 59541 (=BM 1-4), and CFCC 59542 (=BM 1-5).

Notes: Pestalotiopsis jiangsuensis is a species often having one to four tubular apical appendages, which are phylogenetically and morphologically well distinguished from P. foliicola CFCC 54440, P. pinicola KUMCC 19-0183, P. suae CGMCC 3.23546, and P. rosea MFLUCC 12-0258. Although the five strains studied are a sister clade of P. foliicola CFCC 54440, P. pinicola KUMCC 19-0183, P. suae CGMCC 3.23546, and P. rosea MFLUCC 12-0258, the number of apical appendages is quite different. Pestalotiopsis folicola, P. pinicola and P. suae have two to three apical appendages; P. rosea has one to three tubular apical appendages, and some appendages are branched. The strains in this study have one to four apical appendages, and the appendages are unbranched.

Pestalotiopsis funerea has two to four apical appendages, and Pestalotiopsis lawsoniae has two apical appendages. They also have differences with P. jiangsuensis. In addition, P. funerea has a longer basal appendage than that of P. jiangsuensis (5–7) µm vs. (1.4–6.3) µm [43,44].

3.4. Pathogenicity Test

In the experiment of Koch’s postulates, the three representative isolates were pathogenic to Pi. massoniana needles. The development of disease symptoms was observed during a 10-day period. At 5 d, all the Pestalotiopsis jiangsuensis isolates developed gray to gray-brown lesions on wounded needles of Pi. massoniana (Figure 5B–D). At 10 d, the lesion expanded, and in severe cases, the whole needle was necrotic (Figure 5F–H). No symptoms developed on the needles of the control (Figure 5A,E). In this study, the pathogenicity of Pestalotiopsis jiangsuensis is strong; for example, the lesions spread almost to the whole needle after 10 days. It may also relate to its high isolation rate. Pestalotiopsis jiangsuensis was successfully re-isolated from 100% of the inoculated plants and identified based on morphological features and phylogenetic analysis of ITS. Thus, Koch’s postulates had been fulfilled.

4. Discussion

Pestalotiopsis was established by Steyeart (1949) [45] and typified with Pestalotiopsis guepinii Steyaert. Pestalotiopsis sensu lato was classified based on conidia with five-celled, the middle three intermediate colored cells, and hyaline end cells. After that, its taxonomic characteristics gradually changed into conidia spindle-shaped, with five-celled, with colorless or nearly colorless cells at both ends, dark cells in the middle, and one or more branched or unbranched apical appendages arising from the apical cell, with or without basal stalk [20,21,46,47]. The excessive overlap of conidia makes it difficult to identify Pestalotioid species only by morphological characteristics [19]. Although some additional taxonomic features can also be used as the basis for the identification of Pestalotiopsis—such as the pigmentation of median cells, which is an important character to distinguish Pestalotiopsis funerea and P. triseta [23,48]—there are still great limitations [17,22,49]. However, the application of molecular data in the identification of Pestalotiopsis species has greatly improved the accuracy and credibility [22,23,26,50,51]. Pestalotiopsis sensu lato was segregated into three genera by Maharachchikumbura et al. (2014) [15] as Pestalotiopsis sensu stricto, Neopestalotiopsis, and Pseudopestalotiopsis, based on both morphological characteristics and phylogenetic analyses. Gu et al. (2022) [17] identified six new Pestalotiopsis species from Rhododendron, based on phylogenetic analyses of combined ITS, TEF1, and TUB2 genes/region along with morphological characteristics. Maharachchikumbura et al. (2012) [14] identified 23 species of Pestalotiopsis from different host plants in China, including 14 new species, based on phylogenetic analysis of ITS, TEF1, and TUB2 genes/region and morphology. More importantly, concatenating ITS, TUB2, and TEF1 sequences can provide better identification information for Pestalotiopsis [14,52].

The Global Biodiversity Information Facility (https://www.gbif.org/, accessed on 24 November 2023) displays 9320 records of Pestalotiopsis from all over the world, including years and coordinates [53]. The data show that most of them are distributed in Australia, Brazil, China, and the United States. Pestalotiopsis as a plant pathogen has a wide range of symptoms on the hosts, such as withering or chlorosis of leaves, dead shoots or tips, and canker [15]. In Pinus spp., it may be characterized by shoot blight, trunk necrosis, needle blight, and pinecone decay [54]. It is not uncommon that a species of Pestalotiopsis was successfully isolated from needles of Pinus species [34]. For example, Pestalotiopsis neglecta and P. citrina isolated from Pi. sylvestris can cause the needles to turn yellow partially or completely and even cause death of the trees [29,34]. Pestalotiopsis bessey isolated from Pi. halenpesis can cause the entire needles to turn dark gray-brown and eventually cause the death of the trees [55,56]. Pestalotiopsis pini isolated from Pi. Pinea can cause the needles and branches to wither, trunk necrosis, and pinecone rot [54]. Pestalotiopsis is also an endophytic fungus of some Pinus spp., such as P. funerea, and it was isolated from the healthy needles of Pi. pinaster [57].

Interestingly, the pathogen of Pi. massoniana needle blight isolated in a previous study was P. funerea [58], but the pathogen obtained in this study was Pestalotiopsis jiangsuensis, which indicated that the pathogens of the same genus on the same host were diverse. Silva et al. [54] isolated P. disseminata and P. pini from Pi. Pinea, and their results also confirmed this view. Similarly, the same species of Pestalotiopsis can be found on different plant hosts, such as P. funereal, which was isolated from Pi. tabulaeformis, Pi. taeda, and Pi. massoniana [10,27,28]. Pestalotiopsis chamaeropis was isolated from Quercus sp., Castanopsis sp., and Camellia sp. [15,49,59]. However, in the current study the samples were only collected from one site. In future research, the investigation areas should be expanded to study fungal diversity on Pinus spp. and related ecological functions.

5. Conclusions

In this study, we examined five strains, all of which were pathogenic to Pi. massoniana. Combined with morphology, multi-locus phylogenetic analyses, and GCPSR principle, these five strains were identified to be a new species to science, Pestalotiopsis jiangsuensis. This is the first report of needle blight caused by P. jiangsuensis on Pi. massoniana in China and worldwide, and it will provide useful information for future studies on all the phytopathological perspectives of this fungus and the management strategies of this newly emerged disease.

Author Contributions

Conceptualization, L.-H.Z.; methodology, H.L., J.-Y.X. and Y.-Q.B. software, H.L.; validation, H.L.; formal analysis, H.L.; investigation, H.L., J.-Y.X. and Y.-Q.B.; resources, L.-H.Z.; data curation, H.L.; writing—original draft preparation, H.L.; writing—review and editing, D.-W.L.; visualization, H.L. and B.-Y.P.; supervision, D.-W.L.; project administration, L.-H.Z.; funding acquisition, L.-H.Z. All authors have read and agreed to the published version of the manuscript.

Funding

This work was supported by National Key R & D Program of China (2022YFD1401005), and the National Natural Science Foundation of China (grant number 31971659).

Institutional Review Board Statement

Not applicable for studies not involving humans or animals.

Informed Consent Statement

Not applicable.

Data Availability Statement

Data are contained within the article.

Acknowledgments

The authors would like to thank those who provided assistance and advice for this study.

Conflicts of Interest

The authors declare no conflicts of interest.

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Figure 1. Symptoms of needle blight on Pinus massoniana in the field (A–C).

Figure 2. Phylogenetic relationship of Pestalotiopsis jiangsuensis isolates: BM 1-1, BM 1-2, BM 1-3, BM 1-4, and BM 1-5, based on concatenated sequences of ITS, TEF1, and TUB2 genes/region. RA × ML bootstrap support values (ML ≥ 70) and Bayesian posterior probability values (PP ≥ 0.90) were shown at the nodes (ML/PP). Neopestalotiopsis protearum (CBS 114178) is used as an outgroup. Bar = 0.04 substitution per nucleotide position. The sequences from this study are in red. The ex-type strains are in bold.

Figure 3. Pairwise homoplasy index (PHI) test of Pestalotiopsis isolates: BM 1-1, BM 1-2, BM 1-3, BM 1-4, and BM 1-5 and closely related P. foliicola, P. pinicola, P. suae, and P. rosea using both LogDet transformation and splits decomposition. PHI test results (Φw) < 0.05 indicate significant recombination within the data set.

Figure 4. Morphological characteristics of Pestalotiopsis jiangsuensis sp. nov. BM 1-1. (A) Fungal colony on PDA, 5 d growth from above (L) and below (R). (B) Conidiomata and conidial masses. (C) Conidiophores, conidiogenous cells, and conidia. (D) Conidia. Scale bars: (B) = 500 μm, (C,D) = 20 μm.

Figure 5. Pathogenicity of representative isolates of Pestalotiopsis jiangsuensis sp. nov. (BM 1-1, BM 1-2, and BM 1-3) on Pinus massoniana. (A) No symptoms were observed on control pine needles treated with sterile water after 5 days. (B–D) Symptoms on pine needles inoculated with conidial suspensions of BM 1-1, BM 1-2, and BM 1-3 after 5 days, respectively. (E) No symptoms observed on control pine needles treated with sterile water after 10 days. (F–H) Symptoms on pine needles inoculated with conidial suspensions of BM 1-1, BM 1-2, and BM 1-3 after 10 days.

Table 1. Reaction conditions used in PCR amplification and sequencing.

Locus	PCR Primers (Forward/Reverse)	PCR: Thermal Cycles: (Annealing Temperature in Bold)
ITS	ITS5/ITS4	94 °C: 3 min, (94 °C: 45 s, 55 °C: 45 s, 72 °C: 1 min) ×35 cycles, 72 °C: 10 min
TEF1	EF1-728F/EF1-986R	94 °C: 3 min, (94 °C: 45 s, 55 °C: 45 s, 72 °C: 1 min) ×35 cycles, 72 °C: 10 min
TUB2	T1/Bt-2b	94 °C: 3 min, (94 °C: 45 s, 56 °C: 60 s, 72 °C: 1 min) ×35 cycles, 72 °C: 10 min

Table 2. Host, Origin, and GenBank accession numbers of strains of Pestalotiopsis species used for phylogenetic analyses.

Species ^a	Strain Number ^b	Host	Origin	GenBank Accession Number ^c
Species ^a	Strain Number ^b	Host	Origin	ITS	TUB2	TEF1
Pestalotiopsis abietis	CFCC 53011 ^T	Abies fargesii	China	MK397013	MK622280	MK622277
P. adusta	ICMP 6088 ^T	Prunus cerasus	Fiji	JX399006	JX399037	JX399070
P. aggestorum	LC6301 ^T	Camellia sinensis	China	KX895015	KX895348	KX895234
P. anacardiacearum	IFRDCC 2397 ^T	Mangifera indica	China	KC247154	KC247155	KC247156
P. anhuiensis	CFCC 54791 ^T	Cyclobalanopsis glauca	China	ON007028	ON005056	ON005045
P. appendiculata	CGMCC 3.23550 ^T	Rhododendron decorum	China	OP082431	OP185516	OP185509
P. arengae	CBS 331.92 ^T	Arenga undulatifolia	Singapore	KM199340	KM199426	KM199515
P. arceuthobii	CBS 434.65 ^T	Arceuthobium campylopodum	USA	KM199341	KM199427	KM199516
P. australasiae	CBS 114126 ^T	Knightia sp.	New Zealand	KM199297	KM199409	KM199499
P. australis	CBS 114193 ^T	Grevillea sp.	Australia	KM199332	KM199383	KM199475
P. biciliata	CBS 124463 ^T	Platanus × hispanica	Slovakia	KM199308	KM199399	KM199505
P. brachiata	CGMCC 3.18151 ^T	Rhizophora apiculata	Thailand	MK764274	MK764340	MK764318
P. brassicae	CBS 170.26 ^T	Brassica napus	New Zealand	KM199379	-	KM199558
P. camelliae	MFLUCC 12-0277 ^T	Camellia japonica	China	JX399010	JX399041	JX399074
P. camelliae-oleiferae	CSUFTCC 08 ^T	Camellia oleifera	China	OK493593	OK562368	OK507963
P. cangshanensisi	CGMCC 3.23544 ^T	Rhododendron delavayi	China	OP082426	OP185517	OP185510
P. castanopsidis	CFCC 54430 ^T	Castanopsis lamontii	China	OK339732	OK358508	OK358493
P. chamaeropis	CBS 186.71 ^T	Chamaerops humilis	Italy	KM199326	KM199391	KM199473
P. changjiangensis	CFCC 54314 ^T	Castanopsis tonkinensis	China	OK339739	OK358515	OK358500
P. changjiangensis	CFCC 54433	Castanopsis tonkinensis	China	OK339740	OK358516	OK358501
P. chiaroscuro	BRIP 72970 ^T	Sporobolus natalensis	Australia	OK422510	-	-
P. chinensis	MFLUCC 12-0273 ^T	Taxus sp.	China	JX398995	-	-
P. clavata	MFLUCC 12-0268 ^T	Buxus sp.	China	JX398990	JX399025	JX399056
P. colombiensis	CBS 118553 ^T	Eucalyptus urograndis	Colombia	KM199307	KM199421	KM199488
P. cyclobalanopsidis	CFCC 54328 ^T	Cyclobalanopsis glauca	China	OK339735	OK358511	OK358496
P. daliensis	CGMCC 3.23548 ^T	Rhododendron decorum	China	OP082429	OP185511	OP185518
P. dianellae	CBS 143421 ^T	Dianella sp.	Australia	MG386051	MG386164	-
P. digitalis	MFLU 14-0208 ^T	Digitalis purpurea	New Zealand	KP781879	KP781883	-
P. diploclisiae	CBS 115587 ^T	Diploclisia glaucescens	China	KM199320	KM199419	KM199486
P. disseminata	CBS 143904	Persea americana	New Zealand	MH554152	MH554825	MH554587
P. distincta	LC3232 ^T	Camellia sinensis	China	KX894961	KX895293	KX895178
P. diversiseta	MFLUCC12-0287 ^T	Rhododendron sp.	China	JX399009	JX399040	JX399073
P. dracaenae	HGUP 4037 ^T	Dracaena fragrans	China	MT596515	MT598645	MT598644
P. dracaenicola	MFLUCC 18-0913 ^T	Dracaena sp.	Thailand	MN962731	MN962733	MN962732
P. dracontomelon	MFLUCC 10-0149 ^T	Dracontomelon dao	Thailand	KP781877	-	KP781880
P. eleutherococci	HMJAU 60190	Eleutherococcus brachypus	China	OL996127	OL898722	-
P. endophytica	MFLUCC 18-0932 ^T	Magnolia garrettii	Thailand	MW263946	-	MW417119
P. ericacearum	IFRDCC 2439 ^T	Rhododendron delavayi	China	KC537807	KC537821	KC537814
P. etonensis	BRIP 66615 ^T	Sporobolus jacquemontii	Australia	MK966339	MK977634	MK977635
P. ficicola	SAUCC230046 ^T	Ficus microcarpa	China	OQ691974	OQ718749	OQ718691
P. foliicola	CFCC 54440 ^T	Castanopsis faberi	China	ON007029	ON005057	ON005046
P. formosana	NTUCC 17-009 ^T	Neolitsea villosa	China	MH809381	MH809385	MH809389
P. furcata	MFLUCC 12-0054 ^T	Camellia sinensis	Thailand	JQ683724	JQ683708	JQ683740
P. fusoidea	CGMCC 3.23545 ^T	Rhododendron delavayi	China	OP082427	OP185519	OP185512
P. gaultheriae	IFRD 411-014 ^T	Gaultheria forrestii	China	KC537805	KC537819	KC537812
P. gibbosa	NOF 3175 ^T	Gaultheria shallon	Canada	LC311589	LC311590	LC311591
P. grandis-urophylla	E72-04	Eucalyptus grandis	Brazil	KU926710	KU926718	KU926714
P. grevilleae	CBS 114127 ^T	Grevillea sp.	Australia	KM199300	KM199407	KM199504
P. guangxiensis	CFCC 54308 ^T	Quercus griffithii	China	OK339737	OK358513	OK358498
P. guizhouensis	CFCC 57364 ^T	Cyclobalanopsis glauca	China	ON007035	ON005063	ON005052
P. hawaiiensis	CBS 114491 ^T	Leucospermum sp.	USA	KM199339	KM199428	KM199514
P. hispanica	CBS 115391	Eucalyptus globulus	Portugal	MW794107	MW802840	MW805399
P. hollandica	CBS 265.33 ^T	Sciadopitys verticillata	Netherlands	KM199328	KM199388	KM199481
P. humus	CBS 336.97 ^T	Soil	Papua New Guinea	KM199317	KM199420	KM199484
P. hydei	MFLUCC 20-0135 ^T	Litsea petiolata	Thailand	MW266063	MW251112	MW251113
P. iberica	CAA 1004 ^T	Pinus radiata	Spain	MW732248	MW759035	MW759038
P. inflexa	MFLUCC 12-0270 ^T	Unidentified tree	China	JX399008	JX399039	JX399072
P. intermedia	MFLUCC 12-0259 ^T	Unidentified tree	China	JX398993	JX399028	JX399059
P. italiana	MFLUCC 12-0657 ^T	Cupressus glabra	Italy	KP781878	KP781882	KP781881
P. jiangsuensis	CFCC 59538	Pinus massoniana	China	OR533577	OR539191	OR539186
	CFCC 59539			OR533578	OR539192	OR539187
	CFCC 59540			OR533579	OR539193	OR539188
	CFCC 59541			OR533580	OR539194	OR539189
	CFCC 59542			OR533581	OR539195	OR539190
P. jiangxiensis	LC4399 ^T	Camellia sp.	China	KX895009	KX895341	KX895227
P. jinchanghensis	LC6636 ^T	Camellia sinensis	China	KX895028	KX895361	KX895247
P. kaki	KNU-PT-1804 ^T	Diospyros kaki	Korea	LC552953	LC552954	LC553555
P. kandelicola	NCYUCC 19-0355 ^T	Kandelia candel	China	MT560723	MT563100	MT563102
P. kenyana	CBS 442.67 ^T	Coffea sp.	Kenya	KM199302	KM199395	KM199502
P. knightiae	CBS 114138 ^T	Knightia sp.	New Zealand	KM199310	KM199408	KM199497
P. krabiensis	MFLUCC 16-0260 ^T	Pandanus sp.	Thailand	MH388360	MH412722	MH388395
P. lespedezae	SY16E	Pinus armandii	China	EF055205	-	EF055242
P. leucadendri	CBS 121417 ^T	Leucadendron sp.	South Africa	MH553987	MH554654	MH554412
P. licualacola	HGUP4057 ^T	Licuala grandis	China	KC492509	KC481683	KC481684
P. linearis	MFLUCC 12-0271 ^T	Trachelospermum sp.	China	JX398992	JX399027	JX399058
P. linguae	ZHKUCC 22-0159	Pyrrosia lingua	China	OP094104	OP186108	OP186110
P. lithocarpi	CFCC 55100 ^T	Lithocarpus chiungchungensis	China	OK339742	OK358518	OK358503
P. lushanensis	LC4344 ^T	Camelia sp.	China	KX895005	KX895337	KX895223
P. macadamiae	BRIP 63738b ^T	Macadamia integrifolia	Australia	KX186588	KX186680	KX186621
P. malayana	CBS 102220 ^T	Macaranga triloba	Malaysia	KM199306	KM199411	KM199482
P. menhaiensis	CGMCC 3.18250 ^T	Camellia sinensis	China	KU252272	KU252488	KU252401
P. microspora	SS1-033I	Cornus canadensis	Canada	MT644300	-	-
P. monochaeta	CBS 144.97 ^T	Quercus robur	Netherlands	KM199327	KM199386	KM199479
P. montellica	MFLUCC12-0279 ^T	Fagraea bodeni	China	JX399012	JX399043	JX399076
P. nanjingensis	CSUFTCC 16 ^T	Camellia oleifera	China	OK493602	OK562377	OK507972
P. nanningensis	CSUFTCC 10 ^T	Camellia oleifera	China	OK493596	OK562371	OK507966
P. neglecta	TAP1100 ^T	Quercus myrsinaefolia	Japan	AB482220	LC311599	LC311600
P. neolitseae	NTUCC 17-011 ^T	Neolitsea villosa	China	MH809383	MH809387	MH809391
P. novae-hollandiae	CBS 130973 ^T	Banksia grandis	Australia	KM199337	KM199425	KM199511
P. olivacea	SY17A	Pinus armandii	China	EF055215	EF055251	-
P. oryzae	CBS 353.69 ^T	Oryza sativa	Denmark	KM199299	KM199398	KM199496
P. pallidotheae	MAFF 240993 ^T	Pieris japonica	Japan	AB482220	LC311584	LC311585
P. pandanicola	MFLUCC 16-0255 ^T	Pandanus sp.	Thailand	MH388361	MH412723	MH388396
P. papuana	CBS 331.96 ^T	Coastal soil Papua	New Guinea	KM199321	KM199413	KM199491
P. parva	CBS 278.35	Leucothoe fontanesiana	Thailand	KM199313	KM199405	KM199509
P. phoebes	SAUCC230093 ^T	Phoebe zhenna	China	OQ692028	OQ718803	OQ718745
P. photinicola	YB28-2	Mango	China	MK228997	MK360938	MK512491
P. pini	MEAN 1092 ^T	Pinus pinea	Portugal	MT374680	MT374705	MT374693
P. pinicola	KUMCC 19-0183 ^T	Pinus armandii	China	MN412636	MN417507	MN417509
P. portugallica	CBS 393.48 ^T	-	Portugal	KM199335	KM199422	KM199510
P. rhizophorae	MFLUCC 17-0416 ^T	Rhizophora apiculata	Thailand	MK764283	MK764349	MK764327
P. rhododendri	IFRDCC 2399 ^T	Rhododendron sinogrande	China	KC537804	KC537818	KC537811
P. rhodomyrtus	CFCC 55052	Cyclobalanopsis augustinii	China	OM746311	OM839984	OM840083
P. rosarioides	CGMCC 3.23549 ^T	Rhododendron decorum	China	OP082430	OP185513	OP185520
P. rosea	MFLUCC 12-0258 ^T	Pinus sp.	China	JX399005	JX399036	JX399069
P. scoparia	CBS 176.25 ^T	Chamaecyparis sp.	China	KM199330	KM199393	KM199478
P. sequoiae	MFLUCC 13-0399 ^T	Sequoia sempervirens	Italy	KX572339	-	-
P. shaanxiensis	CFCC 54958 ^T	Quercus variabilis	China	ON007026	ON005054	ON005043
P. shorea	MFLUCC 12-0314 ^T	Shorea obtusa	Thailand	KJ503811	KJ503814	KJ503817
P. sichuangensis	CGMCC 3.18244 ^T	Camellia sinensis	China	KX146689	KX146807	KX146748
P. silvicola	CFCC 55296 ^T	Cyclobalanopsis kerrii	China	ON007032	ON005060	ON005049
P. spatholobi	SAUCC231201 ^T	Spatholobus suberectus	China	OQ692023	OQ718798	OQ718740
P. spathulata	CBS 356.86 ^T	Gevuina avellana	Chile	KM199338	KM199423	KM199513
P. spathuliappendiculata	CBS 144035 ^T	Phoenix canariensis	Australia	MH554172	MH554845	MH554607
P. suae	CGMCC3.23546 ^T	Rhododendron delavayi	China	OP082428	OP185521	OP185514
P. telopeae	CBS 114161 ^T	Telopea sp.	Australia	KM199296	KM199403	KM199500
P. terricola	CBS 141.69 ^T	Soil	Pacific Islands	MH554004	MH554680	MH554438
P. thailandica	MFLUCC 17-1616 ^T	Rhizophora apiculata	Thailand	MK764285	MK764351	MK764329
P. trachycarpicola	IFRDCC 2240 ^T	Trachycarpus fortunei	China	JQ845947	JQ845945	JQ845946
P. tumida	CFCC 55158 ^T	Rosa chinensis	China	OK560610	OL814524	OM158174
P. unicolor	MFLUCC 12-0276 ^T	Rhododendron sp.	China	JX398999	JX399030	-
P. verruculosa	MFLUCC 12-0274 ^T	Rhododendron sp.	China	JX398996	-	JX399061
P. vismiae	HHL-DG	Rhizophora stylosa	China	HM535704	HM573246	-
P. yanglingensis	LC4553 ^T	Camellia sinensis	China	KX895012	KX895345	KX895231
P. yunnanensis	HMAS 96359 ^T	Podocarpus macrophyllus	China	AY373375	-	-
Neopestalotiopsis protearum	CBS 114178 ^T	Leucospermum cuneiforme	Zimbabwe	JN712498	KM199463	LT853201

^a Strains isolated from the current study are given in bold. ^T = ex-type culture.^b CFCC = China Forestry Culture Collection Center, China; ICMP = International Collection of Microorganisms from Plants, Auckland, New Zealand; LC = working collection of Lei Cai, housed at the Institute of Microbiology, Chinese Academy of Sciences, Beijing, China; IFRDCC = International Fungal Research and Development Culture Collection, Kunming, Yunnan China; CGMCC = China General Microbiological Culture Collection Center, Beijing, China; CBS = culture collection of the Westerdijk Fungal Biodiversity Institute, Utrecht, The Netherlands; MFLUCC = Mae Fah Luang University Culture Collection, Chiang Rai, Thailand; CSUFTCC = Central South University of Forestry and Technology Culture Collection, Hunan, China; BRIP = Plant Pathology Herbarium, Department of Employment, Economic, Development and Innovation, Queensland, Australia; MFLU = Mae Fah Luang University Herbarium, Thailand; HGUP = Plant Pathology Herbarium of Guizhou University, Guizhou, China; HMJAU = Herbarium of Mycology of Jilin Agricultural University, Jilin, China; SAUCC = Shandong Agricultural University Culture Collection, Taian, Shandong, China; NTUCC = The Department of Plant Pathology and Microbiology, National Taiwan University Culture Collection, Taipei, Taiwan (ROC); NOF = The Fungus Culture Collection of the Northern Forestry Centre, Alberta, Canada; E = The “Coleção de culturas de fungos fitopatogênicos Prof. Maria Menezes”, Universidade Federal Rural de Pernambuco, Recife, Brazil; CAA = culture collection of Artur Alves, housed at Department of Biology, University of Aveiro, Aveiro, Portugal; KNU = Kyungpook National University, Daegu, South Korea; NCYUCC = The National Chiayi University Culture Collection, Jiayi, Taiwan; ZHKUCC = the culture collection of Zhongkai University of Agriculture and Engineering, Guangzhou City, Guangdong, China; TAP = Tamagawa University, Tokyo, Japan; MAFF = Ministry of Agriculture, Forestry and Fisheries, Tsukuba, Ibaraki, Japan; MEAN = Instituto Nacional de Investigação Agrária e Veterinária I. P.; KUMCC = Kunming Institute of Botany Culture Collection, Yunnan, China; HMAS = Mycological Herbarium, Institute of Microbiology, Chinese Academy of Sciences, Beijing, China. ^c ITS = internal transcribed spacer; TUB2 = b-tubulin; TEF1 = translation elongation factor1-α.

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MDPI and ACS Style

Li, H.; Peng, B.-Y.; Xie, J.-Y.; Bai, Y.-Q.; Li, D.-W.; Zhu, L.-H. Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China. J. Fungi 2024, 10, 230. https://doi.org/10.3390/jof10030230

AMA Style

Li H, Peng B-Y, Xie J-Y, Bai Y-Q, Li D-W, Zhu L-H. Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China. Journal of Fungi. 2024; 10(3):230. https://doi.org/10.3390/jof10030230

Chicago/Turabian Style

Li, Hui, Bing-Yao Peng, Jun-Ya Xie, Yu-Qing Bai, De-Wei Li, and Li-Hua Zhu. 2024. "Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China" Journal of Fungi 10, no. 3: 230. https://doi.org/10.3390/jof10030230

APA Style

Li, H., Peng, B. -Y., Xie, J. -Y., Bai, Y. -Q., Li, D. -W., & Zhu, L. -H. (2024). Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China. Journal of Fungi, 10(3), 230. https://doi.org/10.3390/jof10030230

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Pestalotiopsis jiangsuensis sp. nov. Causing Needle Blight on Pinus massoniana in China

Abstract

1. Introduction

2. Materials and Methods

2.1. Field Survey and Fungal Isolation

2.2. Morphological Identification

2.3. Genomic DNA Extraction, PCR, and Sequencing

2.4. Phylogenetic Analyses

2.5. Genealogical Concordance Phylogenetic Species Recognition Analyses

2.6. Pathogenicity Test

3. Results

3.1. Disease Symptoms and Fungal Isolation

3.2. Phylogenetic Analyses

3.3. Taxonomy

3.4. Pathogenicity Test

4. Discussion

5. Conclusions

Author Contributions

Funding

Institutional Review Board Statement

Informed Consent Statement

Data Availability Statement

Acknowledgments

Conflicts of Interest

References

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