This study aims to isolate and identify taxonomic characterization of endophytic fungi from bitter melon in Guangdong province, China. A total of 1172 endophytic fungi are isolated from roots, stems, leaves, flowers, and fruits of healthy plants, and they are classified to 49 taxa based on morphological and molecular features. The results show that endophytic fungi from bitter melon plants exhibit high biodiversity. Arthrinium aureum, A. marii, A. sphaerospermum, Corynascus verrucosus, Curvularia borreriae and C. protuberate have not been recorded in any plants in China. Basidiomycetous endophytes, such as Ceratobasidium sp., and C. cornigerum, are reported in this study for the first time in bitter melon. According to the results of phylogenetic analysis, the rDNA ITS (Internal Transcribed Spacer) sequences can successfully separate species, such as F. solani, F. kyushuense, C. verrucosus, C. globosum, E. rostratum, C. brachyspora, C. verruculosus, C. affinis, P. bougainvilleicola, P. longicolla, P. glabrae, P. verruculosum, P. oxalicum, P. citrinum, P. chermesinum, P. glomerata, A. fumigatus and A. japonicas. Some isolates belonging to A. alternata, C. gloeosporioides, C. cladosporioides, C. brasiliense, C. convolutum, F. proliferatum, F. oxysporum, F. verticillioides, F. equiseti, F. camptoceras and Xylaria, however, require the analysis of others molecular markers to provide better taxonomic resolution. Molecular analyses of rDNA ITS sequences are useful for identification and classification of endophytes of bitter melon, but it is desirable to consider an integrated approach, such as molecular phylogeny, host, colony growth rate, symptoms, and shape of conidia.
Endophytes inter- and/or intra-cellularly colonize healthy living tissues of many host plants, typically without causing any noticeable symptoms of disease [1] - [5] . Endophytic fungi from plants have recently been widely accepted as an important source of drugs [6] , and they are believed to be rich in diversity and to provide an excellent potential source of biologically active novel compounds [7] [8] . Until recently, more than 8600 biologically active compounds have been reported from fungi with various usages [9] .
Bitter melon (Momordica charantia), a medicinal food plant, is known to contain charantin (a steroidal glycoside), vicine (a glycoalkaloid), and polypeptide “p” (a 166 residue insulinomimetic peptide) [10] . Extracts of bitter melon have been found to possess novel bioactive natural products like antibacterial, antifungal, anticancer, antioxidant, antivirus and antidiabetes [11] . The medicinal characteristics of bitter melon may result from the capacity of its endophytes producing biologically active secondary metabolites.
rDNA ITS (Internal Transcribed Spacer) sequences analysis has been widely used in identifying fungi. Sette et al. (2006) identified endophytic fungi from coffee plants at least at the genus level, and the results were in accordance with the previous morphological characterization [12] . Chen et al. (2008) reported that ITS sequences analysis was especially effective in non-sporulating fungi identification and also reduced the impacts of subjective judgement [13] .
The present study aimed to 1) identify endophytic fungi species from bitter melon in Guangdong Province in China, 2) conduct phylogenetic analysis on the ribosomal DNA internal transcribed spacer (ITS) region sequence of endophytes, and 3) collect cultures of endophytic fungi for further screening of the new bioactive compounds.
2. Materials and Methods2.1. Plant Materials
Samples were collected between 2004 and 2009 from healthy bitter melon plants in five sites in Guangdong Province (Site 1: Huadu Station of the Guangzhou Vegetable Science Institute; Site 2: Forecast Station of Crop Diseases and Pests in Zhaoqing city; Site 3: Shitang town, Renhua county, Shaoguan city; Site 4: Xiangqiao district, Chaozhou city; and Site 5: Ducheng town, Yunan county, Yunfu city). Five healthy bitter melon plants (without visible signs of any disease) were collected from the each of the five sites. Each experimental field had fields of bitter melon at least 100 m2 large. The samples were placed in an ice-box and processed within 4 h of collection.
2.2. Fungal Isolation and Cultivation
Surface sterilization was applied as described by Schulz et al. (1993) [14] . The surface-sterilized samples of stem, root, flower, and fruit (all) were cut into 5 × 5 mm fragments. A total of 30 fragments from different tissue type per site were prepared. Five fragments from surface-sterilized leaf discs or other organ segments were evenly placed on a 2% potato dextrose agar (PDA) medium. Fifty microgram streptomycin (AMRESCO)/ml were added to repress bacteria. These plates were incubated at 25˚C for 2 months, and examined periodically. Hyphal tips of the developing fungal colonies were transferred onto new malt extract agar (MEA, 2%) plates. The pure endophytic fungal strains were photographed and preserved in the Institute of Plant Pathology, Zhongkai University of Agriculture and Engineering.
2.3. Checking Surface-Sterilization
The method followed Song et al. (1999) [15] . A viability test was adopted to test the effectiveness of surface- sterilization [14] .
2.4. Identification
Sporulating isolates were identified to genus and possible species using traditional morphological techniques. After subculture of isolates grown on PDA for 1 week at 25˚C, all pure strains were selected for DNA extraction, amplification, and sequencing [16] . DNA samples were checked for purity and integrity by electrophoresis in 1% (w/v) agarose with ethidium bromide (10 mg/mL) in 1 × TAE buffer before storing at 4˚C. Primers ITS4 and ITS5 [17] constructed for molecular phylogenetic studies were used to amplify the ITS region. PCR was carried out as follows: the reaction mix in a total volume of 25 µl contained in font changed 0.2 mM each of the primer pair, 0.2 mM dNTP, 10 - 50 ng DNA, 0.04 U of Taq polymerase (Promega, WI, USA), and 1 × PCR buffer mix. Samples were incubated in a thermal cycler at 94˚C for 3 min, followed by 35 cycles of 94˚C for 30 sec, 55˚C for 30 sec, 72˚C for 1 min; and finally 72˚C for 7 min.
Phylogenetic analysis was based on blast searches of ITS sequence data in the NCBI GenBank database. Sequences were then aligned to other sequences obtained from the GenBank database with Clustal X 1.83 [18] . Phylogenetic analysis was performed with Mega 4.0 [19] using Kimura 2-parameter model with a transition to transversion ration. Phylogenetic trees were built using the neighbor-joining (NJ) methods [20] . Bootstrap tests were performed using 1000 replicates.
3. Results3.1. Species Identification
Fungal endophytes were abundant and diverse in healthy plant tissues of bitter melon. Some of the isolates were non-sporulating and therefore difficult to identify decisively based on morphological characters. Based on morphological and molecular features, a total of 1172 endophytes were separated from bitter melon, and they were subsequently classified to 49 taxa (Table 1).
3.2. Phylogenetic Analysis
One hundred and eighteen strains, representing 49 taxa, were selected to sequence the internal transcribed spacer region (ITS) of nuclear ribosomal DNA.
Among the Fusarium, 30 strains formed five clades (Figure 1). Results showed that five strains of F. solani were clustered together with reference strains of F. solani, forming a unique lineage A1. Results also showed
Endophytes of bitter melon in Guangdong province
Taxon
Sites
Tissues
Ascomycetes
Alternaria alternata
Huadu
Flowers, leaves
Arthrinium aureum
Huadu
Fruits, leaves
A. marii
Huadu
fruits
A. sphaerospermum
Yunfu
Stems
Aspergillus fumigatus
Zhaoqing
Flowers
Annulohypoxylon atroroseum
Zhaoqing
Leaves
A. nitens
Zhaoqing
Leaves
Ascomycete
Huadu
Fruits
Aureobasidium pullulans
Zhaoqing
Fruits
Bionectria ochroleuca
Chaozhou
Leaves
Botryosphaeria rhodina
Zhaoqing
Stems
B. dothidea
Zhaoqing
Fruits
Chaetomium brasiliense
Huadu
Roots
C. globosum
Huadu
Roots
C. hexagonosporum
Huadu
Leaves
C. madrasense
Huadu
Leaves
Cladosporium cladosporioides
Zhaoqing
Leaves, fruits
Huadu
Fruits, leaves
C. oxysporum
Huadu
Fruits
Tianluhu
Leaves
Colletotrichum gloeosporioides
Chaozhou
Stems, leaves
Huadu
Stems, roots
C. capsici
Huadu
Leaves
Corynascus verrucosus
Huadu
Roots
Curvularia borreriae
Shaoguan
Roots
C. eragrostidis
Huadu
Flowers
C. lunata
Huadu
Roots
C. protuberata
Shaoguan
Leaves
C. verruculosa
Huadu
Flowers
Exserohilum rostratum
Huadu
Stems, roots
Fusarium camptoceras
Huadu
Leaves
F. equiseti
Shaoguan
Roots, stems
Huadu
Roots
F. kyushuense
Chaozhou
Roots
Shaoguan
Stems
Zhaoqing
Flowers
F. oxysporum
Shaoguan
Roots
Zhaoqing
Leaves
Huadu
Roots, stems
F. proliferatum
Shaoguan
Stems, roots
F. semitectum
Huadu
Roots
F. solani
Zhaoqing
Flowers, fruits, leaves
Huadu
Roots
F. verticillioides
Shaoguan
Stems
Nigrospora oryzae
Huadu
Stems, fruits
N. panici
Huadu
Leaves
Penicillium chermesinum
Zhaoqing
Fruits
P. oxalicum
Huadu
Roots
Pestalotiopsis palustris
Zhaoqing
Leaves
Phoma glomerata
Huadu
Stems
Phomopsis bougainvilleicola
Huadu
Stems
P. glabrae
Huadu
Stems
Rhizopycnis vagum
Huadu
Fruits
Stemphyllium solani
Zhaoqing
Leaves
Xylaria sp.
Zhaoqing
Leaves
Basidiomycetes
Ceratobasidium sp.
Zhaoqing
Fruits
C. cornigerum
Huadu
Fruits
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 38 taxa of Fusarium, rooted with Penicillium marneffei, Phomopsis longicolla and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 19 taxa of Colletotrichum, rooted with Alternaria alternata, Phomopsis longicolla and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
that three strains of F. proliferatum, one strains of F. oxysporum, and one strains of F. verticillioides were clustered together, forming lineage A2. Seven strains of F. oxysporum were clustered together with reference strains of F. oxysporum and F. proliferatum, forming a unique lineage A3. Four strains of F. kyushuense were clustered together with reference strains of F. kyushuense and F. culmorum, forming a unique lineage A4. Four strains of F. equiseti and five strains of F. camptoceras were clustered together with reference strains of F. equiseti, F. camptoceras and Gibberalla fujikuroi, forming lineage A5.
Among the Colletotrichum, 13 strains formed three clades (Figure 2). Results showed that five strains of C. gloeosporioides were clustered together with reference strains of Glomerella lindemuthiana and C. trifolii, forming a unique lineage A1. Results also showed that three strains of C. gloeosporioides were clustered together with reference strains of C. musae, forming lineage A2. Four strains of C. gloeosporioides were clustered together with reference strains of C. gloeosporioides and G. cingulata, forming a unique lineage A3.
Among the Cladosporium, 12 strains formed three clades (Figure 3). Results showed that one strain of C. cladosporioides formed a unique lineage A1. Six strains of C. cladosporioides were clustered together with reference strains of C. chlorocephalum, C. oxysporum, C. colocasiae, C. tenuissimum, C. cladosporioides and C. gossypiicola, forming lineage A2-1. Five strains of C. cladosporioides were clustered together, forming a unique lineage A2-2.
Among the Alternaria, 8 strains formed one clade (Figure 4). Results showed that eight strains of A. alternata were clustered together with reference strains of A. alternata, A. longipes, A. arborescens, A. tenuissima, forming lineage A.
Among the Corynascus and Chaetomium, 6 strains formed three clades (Figure 5). Results showed that one strain of C. brasiliense, one strain of C. convolutum, and one unidentified strain were clustered together with reference strains of C. sp, forming lineage A1. One strain of C. verrucosus was clustered with reference strains
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 18 taxa of Cladosporium, rooted with Penicillium marneffei, Phomopsis longicolla and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 12 taxa of Alternaria, rooted with Fusarium solani, Penicillium marneffei, Phomopsis longicolla and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
of C. verrucosus, and C. kuwaitiensis, forming a unique lineage A2. Two strains of C. globosum were clustered together with reference strains of C. globosum, and C. bostrychodes, forming a unique lineage A3.
Among the Curvularia, Exserohilum and Bipolaris, 7 strains formed five clades (Figure 6). Results showed that three strains of E. rostratum were clustered with reference strains of E. rostratum, E. pedicellatum, and E. longirostratum, forming a unique lineage A1. One strain of C. brachyspora was clustered with reference strains
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 6 taxa of Corynascus and Chaetomium, rooted with Penicillium marneffei, Phomopsis longicolla and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 17 taxa of Curvularia, Exserohilum and Bipolaris, rooted with Penicillium verruculosum, Phomopsis longicolla and Aspergillus japonicus with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
of C. brachyspora, forming a unique lineage A3. One strain of C. verruculosus was clustered with reference strains of C. verruculosus, forming a unique lineage A4. One strain of C. affinis was clustered together with reference strains of C. affinis, forming a unique lineage A5.
Among the Phomopsis, 4 strains formed three clades (Figure 7). Results showed that one strain of P. bougainvilleicola was clustered with reference strains of P. bougainvilleicola, forming a unique lineage A1. One strain of P. longicolla was clustered with reference strains of P. longicolla, forming a unique lineage A2. Two strains of P. glabrae were clustered with reference strains of P. glabrae, forming a unique lineage A3.
Among the Penicillium, 5 strains formed four clades (Figure 8). Results showed that two strains of P. verruculosum were clustered with reference strains of P. verruculosum, and P. marneffei, forming a unique lineage A1.
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 9 taxa of Phomopsis, rooted with Didymella bryoniae, Phoma glomerata and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 10 taxa of Penicillium, rooted with Phomopsis longicolla, Phoma glomerata and Phoma medicaginis with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
One strain of P. oxalicum was clustered with reference strains of P. oxalicum, forming a unique lineage A2. One strain of P. citrinum was clustered with reference strains of P. citrinum, forming a unique lineage A3. One strain of P. chermesinum was clustered with reference strains of P. chermesinum, forming a unique lineage A4.
Among the Phoma, 7 strains formed three clades (Figure 9). Results showed that six strains of Phoma was clustered with reference strains of P. glomerata, and Didymella bryoniae (anamorph: P. cucurbitacearum), forming a unique lineage A1. One strain of Phoma formed a unique lineage A3.
Among the Aspergillus, 5 strains formed two clades (Figure 10). Results showed that four strains of A. fumigatus were clustered with reference strains of A. fumigatus, forming a unique lineage A1. One strain of A. japonicus was clustered with reference strains of A. japonicus, forming a unique lineage A2.
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 10 taxa of Phoma, rooted with Phomopsis longicolla, Diaporthe phaseolorum and Diaporthe helianthi with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
A neighbor-joining tree was generated based on the 5.8S gene and internal transcribed spacer (ITS1 and ITS2) sequences of 9 taxa of Aspergillus, rooted with Phomopsis longicolla, Phoma medicaginis, Penicillium marneffei and Penicillium verruculosum with Clustal W. The numbers at branches indicated the percentages from 1000 bootstrap replications in which the branch occurred
4. Discussion
Traditional approaches to identifying fungal endophytes rely on microscopic analysis of morphological characteristics. However, significant portions of endophytic isolates consist of sterile mycelia and cannot be identified based on traditional approaches. Phylogenetic analysis of rDNA sequences has been successfully employed for the identification of different morphospecies [21] - [26] . In the present study, there are 49 taxa isolated as endophytic fungi from bitter melon. We conduct molecular phylogenetic analyses of endophytes of bitter melon, and build the phylogenetic tree from ITS sequences between species of the same genus or between the similar genera. Morphological characters, together with DNA sequence information, can be used to identify the endophytic strains.
The endophytic fungi associated with bitter melon comprise a number of cosmopolitan species such as Alternaria alternata, Aspergillus fumigatus, Colletotrichum gloeosporioides and Curvularia lunata. All these genera have been previously isolated as endophytes, not only in Taxus species [25] - [28] , but also in pharmaceutical plants [5] [6] [29] [30] . Arthrinium aureum, A. marii, A. sphaerospermum, Corynascus verrucosus, Curvularia borreriae, C. protuberate, however, have not been recorded in any host plants in China, suggesting that bitter melon harbours novel and diverse fungi. Most fungi reported as endophytes up to date have been identified as ascomycetes and their anamorphs. Basidiomycetous endophytes have only been reported in a few studies [24] [31] - [34] . Basidiomycetous endophytes, such as Ceratobasidium sp., and C. cornigerum, are reported in this study for the first time in bitter melon, and the results show that endophytic fungi from bitter melon exhibit a high biodiversity.
Many phylogenetic studies involving fungi rely on the analysis of ribosomal DNA, in particular the internal transcribed spacer (ITS) regions, to assist in separation at the genus and species levels [35] [36] . Based on phylogenetic analysis of endophytes associated with bitter melon, the ITS sequences successfully separate species, such as F. solani, F. kyushuense, C. verrucosus, C. globosum, E. rostratum, C. brachyspora, C. verruculosus, C. affinis, P. bougainvilleicola, P. longicolla, P. glabrae, P. verruculosum, P. oxalicum, P. citrinum, P. chermesinum, P. glomerata, A. fumigatus and A. japonicas; but on the other hand, some isolates belonging to A. alternata, C. gloeosporioides, C. cladosporioides, C. brasiliense, C. convolutum, F. proliferatum, F. oxysporum, F. verticillioides, F. equiseti, F. camptoceras, Xylaria, require the analysis of others molecular markers to provide better taxonomic resolution. Rivera-Orduña et al. (2011) isolated and identified 116 endophytes of Taxus globosa (Mexican yew), and found that ITS sequences could not provide enough information to analysis of the isolates belonging to the families Xylariaceae and Pleosporomycetidae [28] . In addition, the fungal endophyte zly-17 is identified as a Phomopsis sp., and the phylogenetic analyses based on ITS1, ITS2, and 5.8 ribosomal RNA gene show that this fungal isolate is closely related to P. longicolla (GenBank accession number EU650789).
The present study clarifies phylogenetic relationships among endophytes associated with bitter melon. Molecular analyses of rDNA are proven to be useful for identification of endophytes. In the classification of endophytes, it is necessary to consider an integrated approach, such as molecular phylogeny, host, colony growth rate, symptoms, and shape of conidia.
Acknowledgements
I would like to thank Dr. Tom Hsiang for his comments and suggestions on this manuscript. The research work was granted from Provincial Natural Science Foundation Team Project of Guangdong Province, China (No. E05202480), State technology project item of Guangdong Province, China (No. 20052040102) and Foundation of Zhongkai University of Agriculture and Engineering (No. G3071202).
Cite this paper
Jianghua Huang,Zide Jiang, (2015) Phylogenetic analysis of Endophytes from Bitter Melon (Momordica charantia) in Guangdong Province. Agricultural Sciences,06,609-621. doi: 10.4236/as.2015.66060
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