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Isolation and molecular identification of Trichoderma species from wetland soil and their antagonistic activity against phytopathogens
Journal Pre-proof Isolation and molecular identification of Trichoderma species from wetland soil and their antagonistic activity against phytopathogens Kandasamy Saravanakumar, Myeong-Hyeon Wang PII:
S0885-5765(19)30203-6
DOI:
https://doi.org/10.1016/j.pmpp.2020.101458
Reference:
YPMPP 101458
To appear in:
Physiological and Molecular Plant Pathology
Received Date: 18 July 2019 Revised Date:
31 December 2019
Accepted Date: 5 January 2020
Please cite this article as: Saravanakumar K, Wang M-H, Isolation and molecular identification of Trichoderma species from wetland soil and their antagonistic activity against phytopathogens, Physiological and Molecular Plant Pathology (2020), doi: https://doi.org/10.1016/j.pmpp.2020.101458. This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain. © 2020 Published by Elsevier Ltd.
Kandasamy Saravanakumar :Conceptualization; Data curation; Formal analysis; Investigation; Methodology; Visualization; Roles/Writing – original draft; Writing review & editing. Myeong-Hyeon Wang: Funding acquisition; Project administration; Resources; Software; Supervision; Validation; Writing review & editing
Graphical abstract
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Isolation and molecular identification of Trichoderma species from wetland soil and their
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antagonistic activity against phytopathogens
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Kandasamy Saravanakumar, and Myeong-Hyeon Wang*
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Department of Medical Biotechnology, College of Biomedical Sciences, Kangwon National
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University, Chuncheon, Gangwon do, 24341, Republic of Korea.
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*Corresponding author
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Myeong-Hyeon Wang
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Phone: +82-33-250-6486; Fax: +82-33-241-6480
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Email: [email protected]
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Abstract
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Trichoderma species are known to protect the plants from pathogen infections through
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multifunctions, such as secondary metabolism, mycoparasitism, hyperparasitism, nutrient
24
competition, enzymes and induced systemic resistance (ISR). Herein, we isolated a total of 18
25
Trichoderma strains including nine species such as T. atroviride, T. virens, T. velutinum, T.
26
harzianum, T. asperellum, T. koningiopsis, T. aureoviride, H. lixii, and T. koningii from the soils
27
samples, collected from the wetland ecosystem of South Korea. These strains were screened
28
against the pathogens- Macrophomina phaseolina (MP), Fusarium graminearum (FG), and
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Botrytis cinerea (BC) - by in vitro antagonistic assay. Amongst, T. aureoviride (SKCGW013)
30
showed higher antagonistic activity against the targeted pathogens than other isolates did. The
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strain SKCGW013 was further used for extraction, purification and analysis of the metabolites
32
by using column chromatography (CC) and gas chromatography mass spectroscopy (GC-MS).
33
The expression of secondary metabolites regulatory genes of non-ribosomal peptide synthetase
34
(NRPS), polyketide synthase (PKS) were studied by RT-qPCR. The results showed the presence
35
of eight dominant compounds in the ethyl acetate fraction of the strain SKCGW013 and these
36
compound were then screened by molecular modeling method against phytopathogens. In
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addition, RT-qPCR study revealed the significant expression of metabolites related genes.
38
Further molecular docking study showed that the compounds from strain SKCGW13
39
synergistically inhibited the targeted pathogens. Among the compounds - 2H-Pyran, 3-bromo-2-
40
butoxytetrahydro-, cis - exhibited high docking inhibitory energy against the targeted proteins,
41
FgSwi6 and Bcpmr1 from FG and BC respectively. Overall this study concluded that T.
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aureoviride SKCGW013 was an excellent source for discovery of novel metabolites as bio-
43
control agents as evident by its metabolite profile with antifungal activity. 2
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Keywords: Biocontrol, Trichoderma, Phytopathogens, Enzymes, metabolites.
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1. Introduction
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The ubiquitous fungi Trichoderma species belong to the Ascomycota are present in a wide range
47
of geographical locations. They can be isolated from various ecological sources including soil,
48
water, plant parts and delaying woody materials, etc., by applying the conventional
49
microbiological methods of culture in laboratory or industrial scale production for the generation
50
of various bioactive metabolites and enzymes [1, 2]. Trichoderma strains are rich in the synthesis
51
of various microbial molecules with promising bioactivities [3]. The molecules reported from
52
Trichoderma species act as the elicitor to interact with the phytopathogens or plants to induce the
53
biocontrol activity through the molecular mechanism such as systemic acquired resistance (SAR),
54
and induced systemic resistance (ISR)[4-7]. Moreover, the enzymes and metabolites derived
55
from Trichoderma can synergistically induce the biocontrol activity against various pathogens
56
[8-10]. Universally, it is claimed that Trichoderma species are potent biofertilizer or bio-control
57
agents to enhance the productivity of the agricultural crops [11-14]. In addition, Trichoderma
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strains have recently received a greater attention in bio-nanotechnology, specifically in the
59
synthesis of various bioactive inorganic nanoparticles [15-20].
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The plant diseases caused by various pathogens including the Macrophomina phaseolina
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(MP), Fusarium graminearum (FG), Botrytis cinerea (BC), Rhizoctonia, phythium (RP),
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phytophthora (P) and Curvularia lunata (CL) that lead to significant economic loss in various
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agricultural crops [21]. Trichoderma strains are promising biocontrol against pathogens (MP, FG,
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BC, RP, P and CL) and also stimulating plant growth [22]. They are recognized as economically
65
important fungal groups, involved in biocontrol of various phytopathogens and nematodes 3
66
through mycoparasitism, hyperparasitism, nutrient competition [23]. Being avirulent and
67
endophytic plant symbionts, Trichoderma strains penetrate in plants via roots and trigger
68
beneficial effects through activation of plant innate immunity and nutrients uptake [13, 24].
69
Remarkably, the antibiotic metabolites and enzymes produced from Trichoderma species
70
synergistically inhibit the plant disease incidents [25]. Apart from the agricultural applications,
71
Trichoderma strains are utilized in biotechnology as cell factory for the production various
72
enzymes with industrial importance [26, 27]. Trichoderma strains do produce a number of
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industrially important molecules (for the review see [28]), a few of which are available in the
74
market, such as cellulase from T. reesei, cellobiohydrolase from T. viride and T. reesei, pectin
75
lyases from T. reesei, xylanases from T. reesei and T. konignii and hydrophobin from T. reesei
76
[29]. Moreover, Trichoderma are also known producer of carbohydrate active enzymes
77
(CAZymes), cellulase, exoglucanase, endoglucanase, β-glucosidase, xylanase, pectinase,
78
amylase, glucose isomerase, glucoamylase, protease, phytase, β-glucanase, lipase, phospholipase,
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and lysophospholipase with extensive biotechnological applications; but, the level of enzyme
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production from the naturally occurring strains is low for industrial application. Therefore, some
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of Trichoderma strains are genetically modified to increase the production of targeted molecules
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especially proteins in large scales [30]. The biotechnological and economical importance of
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Trichoderma has increased the interest of searching the novel strains from various ecological
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niche. However, only very few works are demonstrating the isolation and screening of
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biotechnologically important Trichoderma strains from the wetland soils of Republic of Korea.
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Hence, the present work was undertaken on isolation, molecular identification and screening of
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antagonistic Trichoderma from wetland soil, collected from Republic of Korea against various
88
phytopathogens. 4
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2. Materials and Methods
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2.1. Collection of soil samples, isolation and Molecular identification Trichoderma.
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A total of 92 soil samples were collected from two different locations, namely (i) wetland forest,
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Chuncheon
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(37°24'33.64"N; 129°12'12.89"E) (Fig.1). The collected soil samples were kept in the ice box
94
(4°C) and transported to the laboratory of Kangwon National University, Chuncheon for the
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isolation of Trichoderma strains. The strains were isolated using the selective medium modified
96
potato dextrose agar according to the methods described in earlier studies [1, 31]. The strains
97
were purified by repetitive colonies picking and culturing in potato dextrose agar (PDA). Then
98
they were identified by applying the conventional morphological properties and molecular
99
internal transcribed spacer (ITS) and translation elongation factor 1 alpha (tef1a) gene
100
sequencing analysis according to the methods described elsewhere [32-34]. All the Trichoderma
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isolated were preserved in 20% glycerol stock in -80°C.
102
2.3. Screening active biocontrol strain against phytopathogens
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The phytopathogens Macrophomina phaseolina (MP), Fusarium graminearum (FG), and
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Botrytis cinerea (BC) were obtained from Korean culture center of microorganisms, Seoul,
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Republic of Korea. To select the potent biocontrol strain, a total of 18 Trichoderma strains were
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screened against the three phytopathogens by antagonist assay described earlier [35, 36]. In brief,
107
the 5 mm of the growing edge of the Trichoderma and phytopathogens were placed on opposite
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direction of PDA plates and incubated at 27±2 °C in incubator for 5 days. Then the growth
109
inhibition was measured using the roller and percentage of the inhibition rate was calculated
110
using the formula described elsewhere [8, 36, 37] as I = (Control-Test)/control x 100, where I-
si
(37°51'19.84"N;
127°44'50.28"E), (ii)
5
coastal wetland,
Gangwan
do
111
percent of inhibition, control-pathogens radial growth (cm), and test-pathogens radial growth
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(cm) in dual culture plate. Followed by the cell wall degrading enzyme activity from the potent
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antagonist strain was analyzed using the methods reported elsewhere [38, 39].
114
2.4. Extraction and GC-MS analysis of secondary metabolites
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Among the tested Trichoderma strains, T. aureoviride (SKCGW013) was selected as potent
116
biocontrol strain and used for the extraction of metabolites. The strain was cultured in
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Trichoderma biomass production medium described elsewhere [8] at 28±2°C in 180 rpm for 10
118
days in shaking incubator. After the incubation period the extracellular products and fungal
119
mycelia were separated by filtration using the Whatman No. 4 and then the extracellular products
120
was extracted with 250 ml of ethyl acetate for overnight at 180 rpm. The ethyl acetate phase and
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water phase were separated using a separating funnel. The ethyl acetate phase containing
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metabolites was concentrated using a rotary evaporator at 40 °C. Finally the ethyl acetate extract
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was re-extracted and then subjected to the gas chromatography and mass spectrophotometry
124
(GS-MS; HP Agilent Technology, 7890A California, USA) analyses. Secondary metabolites
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from the extract of T. aureoviride (SKCGW013) were identified by matching the GC-MS results
126
with electronic searches of the National Institute of Standard and Technology (NIST) GC-MS
127
chromatogram and mass electronic library W8N05ST.L.
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2.5. Antifungal activity of metabolites
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The antifungal activity of T. aureoviride extracts (TAE) was tested against the targeted fungal
130
pathogen (FG) in PDA plates according to the methods described earlier [8]. In brief, the
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different concentrations of TAE (50-500 µg.mL-1) was sterilized by filtration and then
132
incorporated into cooled PDA. After solidification, the FG was inoculated on the PDA medium, 6
133
incorporated with TAE and the plates were incubated in 27±2 °C for 4 days and then the
134
percentage of growth inhibition was measured using the standard formula by comparing the
135
growth of the FG on PDA plates containing with or without TAE and the results are presented as
136
FG growth inhibition (%) calculated according to the formula described above.
137
2.6. Virtual screening of active metabolites
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The protein FgSwi6 from FG is known to be involved in the growth, pathogenicity carbendazim
139
sensitivity, cellulose utilization, lithium tolerance, deoxynivalenol production and virulence of
140
filamentous fungus FG [40]. Another protein Bcpmr1 from BC is also known to be involved in
141
the pathogenicity and growth of BC [41, 42]. These two proteins were targeted using the
142
metabolites identified from TAE by applying the computational modeling study. For the
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computational study, the 3D structure of the proteins, FgSwi6 and Bcpmr1 was prepared by
144
retrieving their sequences from the NCBI (https://www.ncbi.nlm.nih.gov/protein/). These protein
145
sequences
146
(https://www.swissmodel.expasy.org/). The proteins were then pretreated according to the
147
protocols described earlier [43]. The structure of the ligands (compounds identified from TAE),
148
such as 6-Pentyl-2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept-5-ene-2,3-
149
dicarboxylic
150
ethanamine,
151
phenylpropinoic acid were generated using the ACD/ChemSketch using the canonical SMILES
152
retrieved from the PubChem (https://www.ncbi.nlm.nih.gov/pccompound). The ligand and
153
receptor interactions based on their docking energy score were measured by computational
154
modelling using the ArgusLab 4.0.1 (Mark Thompson and Planaria Software LLC). Finally the
were
used
acid,
to
generate
2H-Pyran,
the
3D
structure
using
3-bromo-2-butoxytetrahydro-,
cis,
the
SWISS
2,4-Cyclopentadiene-1-
1,3,3-Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene,
7
MODEL
and
3-
155
interactions between the receptor and ligands were observed by BIOVIA Discovery Studio 2016
156
(Accelrys Software Inc., San Diego, CA, USA).
157
3. Results and discussion
158
3.1. Isolation and identification of Trichoderma
159
Generally the identification of the Trichoderma spp. usually accepted based on the two DNA
160
gene fragment sequence analysis, while the new Trichoderma spp. can be accepted by at least
161
three DNA barcode fragments analysis [44-46]. Thus present work a total of 18 isolates divided
162
into nine species of Trichoderma were isolated from two different sampling sites of Republic of
163
Korea (Fig.1) and identified based on two DNA gene sequencing analysis including internal
164
transcribed spacer (ITS) and translation elongation factor 1 alpha (tef 1α) based NCBI blast
165
analysis (Fig.2). However, a number of the classification studies have shown that the individual
166
sequence such as ITS, or tef- 1α gene sequences based phylogenic tree was not able to
167
distinguish all Trichoderma spp. Thus combination of multi-loci sequences based phylogenic
168
tree analysis is suggested for better distribution of Trichoderma spp. [47, 48]. Therefore, in the
169
present work was contracted the phylogenetic tree using the concatenated dataset of ITS- tef 1α
170
inferred by maximum parsimony method [49]. The same or closely related species were
171
clustered on a clade on the resulting tree and the test and conference taxa was compared clearly
172
according to earlier report [1, 2, 46, 50, 51]. The present results revealed the similarities between
173
Trichoderma species while the out-group sequence of Nectria berolinensis formed the non-
174
similarity clusters. Interesting the T. harzianum was formed a group of cluster in association with
175
reference sequence while another group was formed for same clades association with other
176
species such as T. virens, T. velutinum and Hypocrea lixii. Similar results were obtained for the 8
177
Viride clades, which indicated the similarity of the species within clades of Trichoderma species.
178
Although, the concatenated dataset of ITS- tef 1α of Trichoderma spp. formed the similar groups
179
according to their species but in case of clades were formed the two different group that's
180
indicated the difference within the clades (Fig.2). For instance, the present study observed two
181
different cluster for Viride and Green/Harzianum from the concatenated dataset of ITS- tef 1α
182
inferred by maximum parsimony tree, which indicated the requirement of further depth
183
molecular assessment for better understanding of the Trichoderma taxonomy. Among the two
184
sites of the coastal area, the site II showed high species diversity and richness (Table.1). The
185
dominant species recorded were T. harzianum. T. atroviride, T. virens, T. velutinum,
186
T.harzianum, T. asperellum, T. koningiopsis, T. aureoviride, and T. koningii (Table 1).
187
3.2. Screening of active biocontrol strains
188
Trichoderma isolates were tested against three phytopathogens (MP, FG and BC) by
189
antagonistic assay. All the strains showed the potential antagonist activity against the targeted
190
pathogens. Among the strains, T. aureoviride (SKCGW013) showed a high inhibition activity
191
against MP (92.5%), FG (94.5%) and BC (89.32%) (Fig.3). Similarly, earlier reports also
192
evidenced the potent inhibitory effect of Trichoderma on pathogens such as Botrytis cinerea[52],
193
Fusarium graminearum [25, 53] and Macrophomina phaseolina [54] through the production of
194
antibiotic metabolites and enzymes mediated competition for nutrients and space[55, 56].
195
Moreover, the strain SKCGW013 was showed the higher enzyme activity such as chitinase
196
(71.21±1.44%), cellulase (68.45±2.32%), protease (48.65±0.12%) and β-(1-3) glucanase
197
(78.15±1.84%) and it was higher than other strains tested in this study. Further study analyzed
198
the metabolites profile of the strain SKCGW013 by applying the chromatography assay. The
199
results showed a total of the 185 secondary metabolites including the polyketides, esters, nitriles, 9
200
alkanes, benzenes, olefins, acids, alcohols and aldehydes in the ethyl acetate extract of
201
SKCGW013 (Fig.4a). Similarly, Trichoderma strains are known to produce chemically
202
diversified antifungal metabolites as the biological weapon against various phytopathogens [57-
203
60]. The antifungal activity of unbounded metabolites of Trichoderma was then tested against
204
fungal pathogen FG. The results showed significant inhibition of FG at the dose depended
205
manner (Fig.4b&c). Similarly the crude extracts of Trichoderma strains are reported to inhibit
206
the growth of F. graminearum and F. oxysporum f. sp. cucumerinum in the PDA plates [8, 25].
207
Thus the present results confirmed the biocontrol potential and stability of unbounded
208
compounds of Trichoderma against phytopathogens.
209
3.3. GC-MS based identification of dominant compounds and computational studies
210
Based on the chromatography, the dominant metabolites from TAE of SKCGW013 were
211
identified as 6-Pentyl-2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept-5-
212
ene-2,3-dicarboxylic acid, 2H-Pyran, 3-bromo-2-butoxytetrahydro-, cis, 2,4-Cyclopentadiene-1-
213
ethanamine,
214
phenylpropinoic acid (Fig.5a). These compounds were selected for the molecular inhibitory
215
interaction towards the proteins - FgSwi6 from the FG [40] and Bcpmr1 from BC [41, 42] by
216
using the computation approach. The docking results showed that all the tested compounds
217
showed good docking score against the targeted proteins, evidencing the synergetic antifungal
218
activity of metabolites from TAE (Table 2). Among the compounds,
219
butoxytetrahydro-, cis (Fig. 5b) displayed higher interaction and inhibitory capacity against the
220
targeted proteins, as indicated by promising docking energy of -8.812 Kcal/mol against FgSwi6
221
and that of -9.808 against Bcpmr1. The active compound 2H-Pyran, 3-bromo-2-
222
butoxytetrahydro-, cis
1,3,3-Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene,
inhibited the expression of 10
and
3-
2H-Pyran, 3-bromo-2-
FgSwi6 by establishing the bond with
223
aliphatic hydrophobic side chain Ile 590, Ile725, Ile 600, Leu593, Ile 368, Ala 724, Leu 362, Ile
224
721, Met 711, Met 677, Val 695 and Ala 676, aromatic hydrophobic side chain Phe 718, and
225
polar neutral side chain Thr 678 (Fig.6a-b). In the case of Bcpmr1, the active compound
226
interacted through bond with aliphatic hydrophobic side chain Leu 436, Leu 435, Leu 396, Ile
227
400, Val 438, and Leu439, and electrically charged side chain Arg 397 (Fig.6c-d). Similar kind
228
of the molecular docking approaches are previously applied to screen the active compounds from
229
Trichoderma against fungal pathogens, such as F. graminearum and F. oxysporum [8, 25]
230
3.4. qRT-PCR Analysis of the secondary metabolites regulatory genes
231
The ketosynthase domain of PKSI gene and adenylation domain of NRPS gene were
232
detected through PCR amplification as these genes are involved in the antimicrobial activity [61].
233
The qRT-PCR results indicated that both genes were expressed but the level of expression was
234
higher in NRPS gene (relative gene expression 2.41) than that in PKS1gene (relative gene
235
expression 9.22). The gene expression indicated the presence of metabolites in TAE belonging
236
to NRPS and PKS1 families that resulted in enhanced antifungal activity [62]. Similarly, the
237
previous results have evidenced the correlation between the expression of the NRPS and PKS1 in
238
the endophytic fungi and their bioactivities including antimicrobial, biomedical and biocontrol
239
activity [63-65].
240
4. Conclusion
241
This work reported the potential of newly isolated T. aureoviride (SKCGW013) on the inhibition
242
of phytopathogens (MP, FG, and BC). The strain synthesised novel metabolites such as 6-Pentyl-
243
2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept-5-ene-2,3-dicarboxylic acid,
244
2H-Pyran,
3-bromo-2-butoxytetrahydro-,
cis, 11
2,4-Cyclopentadiene-1-ethanamine,
1,3,3-
245
Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene, and 3-phenylpropinoic acid as evident
246
by the preliminary metabolism analysis. This calls for critical study on transcriptomes to
247
understand molecular mechanisms adapted by Trichoderma strain for antifungal activity.
248
Therefore, further study will be focused on purification and molecular mechanism of synthesis
249
for the secondary metabolites, produced by T. aureoviride (SKCGW013).
250
Conflict of interest
251
The authors declare that they have no conflict of interest
252
Acknowledgment
253
This work was supported Korea Research Fellowship Program through the National Research
254
Foundation of Korea (NRF) funded by the Ministry of Science, ICT (2017H1D3A1A01052610).
255
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424
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Table 1. Description of List of Trichoderma strains collected by this study and their sources Strain code
Culture collection
Identification
Source
KNUP001
NCBI accession ITS1,ITS2 tef-α MG552067 MN513281
CMTCC KNU001
Soil, Wetland forest, Chuncheon
KNUP002
MG552068
MN513282
CMTCC KNU002
SKCGW001
MG552069
MN513283
CMTCC KNU003
SKCGW002
MG552070
MN513284
CMTCC KNU004
SKCGW003
MG552071
MN513285
CMTCC KNU005
SKCGW004
MG940956
MN513286
CMTCC KNU006
SKCGW005
MG940957
MN513287
CMTCC KNU007
SKCGW006
MG940958
MN513288
CMTCC KNU008
SKCGW007
MG940959
MN513289
CMTCC KNU009
SKCGW008
MG940960
MN513290
CMTCC KNU010
SKCGW009
MG940961
MN513291
CMTCC KNU011
SKCGW010
MG940962
MN513292
CMTCC KNU012
SKCGW011
MG940963
MN513293
CMTCC KNU013
SKCGW012
MG940964
MN513294
CMTCC KNU014
Trichoderma atroviride Trichoderma virens Trichoderma velutinum Trichoderma harzianum Trichoderma asperellum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma koningiopsis Trichoderma koningiopsis Trichoderma
Soil, Wetland forest, Chuncheon Sediemnt, Coastal wetland, Gangwan Sediemnt, Coastal wetland, Gangwan Sediemnt, Coastal wetland, Gangwan Sediemnt, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan
SKCGW013
MG940965
MN513295
CMTCC KNU015
SKCGW014 SKCGW015
MG940966 MG940967
MN513296 MN513297
CMTCC KNU016 CMTCC KNU017
SKCGW016
MG940968
MN513298
CMTCC KNU018
harzianum Trichoderma aureoviride Hypocrea lixii Trichoderma koningiopsis Trichoderma koningii
Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan
Table 2. Interactions between Trichoderma derived compounds and pathogenicity related protein bcpmr1 of Botrytis cinerea and FgSwi6 of Fusarium graminearum. S.no
1 3 5
11.089 24.271
6-Pentyl-2H-pyran-2-one Propionamide
Docking Score (Kcal/mol) Molecular Weight (g/mol) FgSwi6 Bcpmr1 166.22 -8.677 -9.001 73.095 -5.639 -6.192
23.341
2-Aminooctane
129.247
Retention Compound Name time
6 25.554 9 10.382 10 16.287 11
12
17.610 33.302
Bicyclo[2.2.1]hept-5-ene2,3-dicarboxylic acid 182.175 2H-Pyran, 3-bromo-2butoxytetrahydro-, cis 237.13 2,4-Cyclopentadiene-1ethanamine. 109.17 1,3,3-Trimethyl-2(hydroxymethyl)-5-hydroxy1-cyclohexene 170.25 3-phenylpropinoic acid 150.17
-8.356
-9.075
-8.460
-8.344
-8.812
-9. 808
-7.17
-8.485
-8.393 -8.411
-7.683 -9.721
Fig.1. Soil samples collected from two different wetland locations. (i) Soil from wetland forest, Chuncheon si (37°51'19.84"N; 127°44'50.28"E), 2. Sediment from Coastal wetland, Gangwan do (37°24'33.64"N; 129°12'12.89"E) (Sourcehttps://www.google.com/maps/place/Chuncheonsi,+Gangwon-do)
Fig.2. Phylogenetic tree inferred by neighbor joining analysis performed on the ITS-Tef 1α concatenated sequences dataset of Trichoderma spp.
Fig.3. Antagonistic activity of newly isolated Trichoderma strains against three different plant pathogens on PDA (a), percentage of pathogens growth inhibition (b), MP- Macrophomina phaseolina, FG- Fusarium graminearum, BC- Botrytis cinerea.
Fig.4. Distribution of secondary metabolites profile from unbounded extract TAE (a), Antifungal activity of unbounded metabolites derived from Trichoderma sp. (b) and % of inhibition of FG at different concentration of Trichoderma extracts (c).
Fig.5. Chromatography of the potent antifungal compound isolated from T. aureoviride at retention time of 11.089, 24.271, 23.341, 25.554, 10.382, 16.287, 17.610, 33.302 min corresponding to 6-Pentyl-2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept5-ene-2,3-dicarboxylic acid, 2H-Pyran, 3-bromo-2-butoxytetrahydro-, cis, 2,4-Cyclopentadiene1-ethanamine, 1,3,3-Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene, and 3phenylpropinoic acid (a), the potent antifungal compound structure of 2H-Pyran, 3-bromo-2butoxytetrahydro-, cis, (b)
Fig.6. 3D and 2D structure demonstrate the interaction between 2H-Pyran, 3-bromo-2butoxytetrahydro-, cis with FgSwi6 from filamentous fungus Fusarium graminearum (a, b) and Bcpmr1 from B. cinera (c,d).
Highlights • This work reported the potent biocontrol strain from wetland soil of Republic of Korea. • A total of nine Trichoderma species was isolated with potent biocontrol properties • T. auroviride (SKCGW013) inhibited the growth of various phytopathogens • Metabolites from the T. auroviride induced biocontrol activity synergistically
Declaration of interests ☐ The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper.
S0885-5765(19)30203-6
DOI:
https://doi.org/10.1016/j.pmpp.2020.101458
Reference:
YPMPP 101458
To appear in:
Physiological and Molecular Plant Pathology
Received Date: 18 July 2019 Revised Date:
31 December 2019
Accepted Date: 5 January 2020
Please cite this article as: Saravanakumar K, Wang M-H, Isolation and molecular identification of Trichoderma species from wetland soil and their antagonistic activity against phytopathogens, Physiological and Molecular Plant Pathology (2020), doi: https://doi.org/10.1016/j.pmpp.2020.101458. This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain. © 2020 Published by Elsevier Ltd.
Kandasamy Saravanakumar :Conceptualization; Data curation; Formal analysis; Investigation; Methodology; Visualization; Roles/Writing – original draft; Writing review & editing. Myeong-Hyeon Wang: Funding acquisition; Project administration; Resources; Software; Supervision; Validation; Writing review & editing
Graphical abstract
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Isolation and molecular identification of Trichoderma species from wetland soil and their
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antagonistic activity against phytopathogens
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Kandasamy Saravanakumar, and Myeong-Hyeon Wang*
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Department of Medical Biotechnology, College of Biomedical Sciences, Kangwon National
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University, Chuncheon, Gangwon do, 24341, Republic of Korea.
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*Corresponding author
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Myeong-Hyeon Wang
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Phone: +82-33-250-6486; Fax: +82-33-241-6480
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Email: [email protected]
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Abstract
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Trichoderma species are known to protect the plants from pathogen infections through
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multifunctions, such as secondary metabolism, mycoparasitism, hyperparasitism, nutrient
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competition, enzymes and induced systemic resistance (ISR). Herein, we isolated a total of 18
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Trichoderma strains including nine species such as T. atroviride, T. virens, T. velutinum, T.
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harzianum, T. asperellum, T. koningiopsis, T. aureoviride, H. lixii, and T. koningii from the soils
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samples, collected from the wetland ecosystem of South Korea. These strains were screened
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against the pathogens- Macrophomina phaseolina (MP), Fusarium graminearum (FG), and
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Botrytis cinerea (BC) - by in vitro antagonistic assay. Amongst, T. aureoviride (SKCGW013)
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showed higher antagonistic activity against the targeted pathogens than other isolates did. The
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strain SKCGW013 was further used for extraction, purification and analysis of the metabolites
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by using column chromatography (CC) and gas chromatography mass spectroscopy (GC-MS).
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The expression of secondary metabolites regulatory genes of non-ribosomal peptide synthetase
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(NRPS), polyketide synthase (PKS) were studied by RT-qPCR. The results showed the presence
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of eight dominant compounds in the ethyl acetate fraction of the strain SKCGW013 and these
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compound were then screened by molecular modeling method against phytopathogens. In
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addition, RT-qPCR study revealed the significant expression of metabolites related genes.
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Further molecular docking study showed that the compounds from strain SKCGW13
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synergistically inhibited the targeted pathogens. Among the compounds - 2H-Pyran, 3-bromo-2-
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butoxytetrahydro-, cis - exhibited high docking inhibitory energy against the targeted proteins,
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FgSwi6 and Bcpmr1 from FG and BC respectively. Overall this study concluded that T.
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aureoviride SKCGW013 was an excellent source for discovery of novel metabolites as bio-
43
control agents as evident by its metabolite profile with antifungal activity. 2
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Keywords: Biocontrol, Trichoderma, Phytopathogens, Enzymes, metabolites.
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1. Introduction
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The ubiquitous fungi Trichoderma species belong to the Ascomycota are present in a wide range
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of geographical locations. They can be isolated from various ecological sources including soil,
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water, plant parts and delaying woody materials, etc., by applying the conventional
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microbiological methods of culture in laboratory or industrial scale production for the generation
50
of various bioactive metabolites and enzymes [1, 2]. Trichoderma strains are rich in the synthesis
51
of various microbial molecules with promising bioactivities [3]. The molecules reported from
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Trichoderma species act as the elicitor to interact with the phytopathogens or plants to induce the
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biocontrol activity through the molecular mechanism such as systemic acquired resistance (SAR),
54
and induced systemic resistance (ISR)[4-7]. Moreover, the enzymes and metabolites derived
55
from Trichoderma can synergistically induce the biocontrol activity against various pathogens
56
[8-10]. Universally, it is claimed that Trichoderma species are potent biofertilizer or bio-control
57
agents to enhance the productivity of the agricultural crops [11-14]. In addition, Trichoderma
58
strains have recently received a greater attention in bio-nanotechnology, specifically in the
59
synthesis of various bioactive inorganic nanoparticles [15-20].
60
The plant diseases caused by various pathogens including the Macrophomina phaseolina
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(MP), Fusarium graminearum (FG), Botrytis cinerea (BC), Rhizoctonia, phythium (RP),
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phytophthora (P) and Curvularia lunata (CL) that lead to significant economic loss in various
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agricultural crops [21]. Trichoderma strains are promising biocontrol against pathogens (MP, FG,
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BC, RP, P and CL) and also stimulating plant growth [22]. They are recognized as economically
65
important fungal groups, involved in biocontrol of various phytopathogens and nematodes 3
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through mycoparasitism, hyperparasitism, nutrient competition [23]. Being avirulent and
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endophytic plant symbionts, Trichoderma strains penetrate in plants via roots and trigger
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beneficial effects through activation of plant innate immunity and nutrients uptake [13, 24].
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Remarkably, the antibiotic metabolites and enzymes produced from Trichoderma species
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synergistically inhibit the plant disease incidents [25]. Apart from the agricultural applications,
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Trichoderma strains are utilized in biotechnology as cell factory for the production various
72
enzymes with industrial importance [26, 27]. Trichoderma strains do produce a number of
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industrially important molecules (for the review see [28]), a few of which are available in the
74
market, such as cellulase from T. reesei, cellobiohydrolase from T. viride and T. reesei, pectin
75
lyases from T. reesei, xylanases from T. reesei and T. konignii and hydrophobin from T. reesei
76
[29]. Moreover, Trichoderma are also known producer of carbohydrate active enzymes
77
(CAZymes), cellulase, exoglucanase, endoglucanase, β-glucosidase, xylanase, pectinase,
78
amylase, glucose isomerase, glucoamylase, protease, phytase, β-glucanase, lipase, phospholipase,
79
and lysophospholipase with extensive biotechnological applications; but, the level of enzyme
80
production from the naturally occurring strains is low for industrial application. Therefore, some
81
of Trichoderma strains are genetically modified to increase the production of targeted molecules
82
especially proteins in large scales [30]. The biotechnological and economical importance of
83
Trichoderma has increased the interest of searching the novel strains from various ecological
84
niche. However, only very few works are demonstrating the isolation and screening of
85
biotechnologically important Trichoderma strains from the wetland soils of Republic of Korea.
86
Hence, the present work was undertaken on isolation, molecular identification and screening of
87
antagonistic Trichoderma from wetland soil, collected from Republic of Korea against various
88
phytopathogens. 4
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2. Materials and Methods
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2.1. Collection of soil samples, isolation and Molecular identification Trichoderma.
91
A total of 92 soil samples were collected from two different locations, namely (i) wetland forest,
92
Chuncheon
93
(37°24'33.64"N; 129°12'12.89"E) (Fig.1). The collected soil samples were kept in the ice box
94
(4°C) and transported to the laboratory of Kangwon National University, Chuncheon for the
95
isolation of Trichoderma strains. The strains were isolated using the selective medium modified
96
potato dextrose agar according to the methods described in earlier studies [1, 31]. The strains
97
were purified by repetitive colonies picking and culturing in potato dextrose agar (PDA). Then
98
they were identified by applying the conventional morphological properties and molecular
99
internal transcribed spacer (ITS) and translation elongation factor 1 alpha (tef1a) gene
100
sequencing analysis according to the methods described elsewhere [32-34]. All the Trichoderma
101
isolated were preserved in 20% glycerol stock in -80°C.
102
2.3. Screening active biocontrol strain against phytopathogens
103
The phytopathogens Macrophomina phaseolina (MP), Fusarium graminearum (FG), and
104
Botrytis cinerea (BC) were obtained from Korean culture center of microorganisms, Seoul,
105
Republic of Korea. To select the potent biocontrol strain, a total of 18 Trichoderma strains were
106
screened against the three phytopathogens by antagonist assay described earlier [35, 36]. In brief,
107
the 5 mm of the growing edge of the Trichoderma and phytopathogens were placed on opposite
108
direction of PDA plates and incubated at 27±2 °C in incubator for 5 days. Then the growth
109
inhibition was measured using the roller and percentage of the inhibition rate was calculated
110
using the formula described elsewhere [8, 36, 37] as I = (Control-Test)/control x 100, where I-
si
(37°51'19.84"N;
127°44'50.28"E), (ii)
5
coastal wetland,
Gangwan
do
111
percent of inhibition, control-pathogens radial growth (cm), and test-pathogens radial growth
112
(cm) in dual culture plate. Followed by the cell wall degrading enzyme activity from the potent
113
antagonist strain was analyzed using the methods reported elsewhere [38, 39].
114
2.4. Extraction and GC-MS analysis of secondary metabolites
115
Among the tested Trichoderma strains, T. aureoviride (SKCGW013) was selected as potent
116
biocontrol strain and used for the extraction of metabolites. The strain was cultured in
117
Trichoderma biomass production medium described elsewhere [8] at 28±2°C in 180 rpm for 10
118
days in shaking incubator. After the incubation period the extracellular products and fungal
119
mycelia were separated by filtration using the Whatman No. 4 and then the extracellular products
120
was extracted with 250 ml of ethyl acetate for overnight at 180 rpm. The ethyl acetate phase and
121
water phase were separated using a separating funnel. The ethyl acetate phase containing
122
metabolites was concentrated using a rotary evaporator at 40 °C. Finally the ethyl acetate extract
123
was re-extracted and then subjected to the gas chromatography and mass spectrophotometry
124
(GS-MS; HP Agilent Technology, 7890A California, USA) analyses. Secondary metabolites
125
from the extract of T. aureoviride (SKCGW013) were identified by matching the GC-MS results
126
with electronic searches of the National Institute of Standard and Technology (NIST) GC-MS
127
chromatogram and mass electronic library W8N05ST.L.
128
2.5. Antifungal activity of metabolites
129
The antifungal activity of T. aureoviride extracts (TAE) was tested against the targeted fungal
130
pathogen (FG) in PDA plates according to the methods described earlier [8]. In brief, the
131
different concentrations of TAE (50-500 µg.mL-1) was sterilized by filtration and then
132
incorporated into cooled PDA. After solidification, the FG was inoculated on the PDA medium, 6
133
incorporated with TAE and the plates were incubated in 27±2 °C for 4 days and then the
134
percentage of growth inhibition was measured using the standard formula by comparing the
135
growth of the FG on PDA plates containing with or without TAE and the results are presented as
136
FG growth inhibition (%) calculated according to the formula described above.
137
2.6. Virtual screening of active metabolites
138
The protein FgSwi6 from FG is known to be involved in the growth, pathogenicity carbendazim
139
sensitivity, cellulose utilization, lithium tolerance, deoxynivalenol production and virulence of
140
filamentous fungus FG [40]. Another protein Bcpmr1 from BC is also known to be involved in
141
the pathogenicity and growth of BC [41, 42]. These two proteins were targeted using the
142
metabolites identified from TAE by applying the computational modeling study. For the
143
computational study, the 3D structure of the proteins, FgSwi6 and Bcpmr1 was prepared by
144
retrieving their sequences from the NCBI (https://www.ncbi.nlm.nih.gov/protein/). These protein
145
sequences
146
(https://www.swissmodel.expasy.org/). The proteins were then pretreated according to the
147
protocols described earlier [43]. The structure of the ligands (compounds identified from TAE),
148
such as 6-Pentyl-2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept-5-ene-2,3-
149
dicarboxylic
150
ethanamine,
151
phenylpropinoic acid were generated using the ACD/ChemSketch using the canonical SMILES
152
retrieved from the PubChem (https://www.ncbi.nlm.nih.gov/pccompound). The ligand and
153
receptor interactions based on their docking energy score were measured by computational
154
modelling using the ArgusLab 4.0.1 (Mark Thompson and Planaria Software LLC). Finally the
were
used
acid,
to
generate
2H-Pyran,
the
3D
structure
using
3-bromo-2-butoxytetrahydro-,
cis,
the
SWISS
2,4-Cyclopentadiene-1-
1,3,3-Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene,
7
MODEL
and
3-
155
interactions between the receptor and ligands were observed by BIOVIA Discovery Studio 2016
156
(Accelrys Software Inc., San Diego, CA, USA).
157
3. Results and discussion
158
3.1. Isolation and identification of Trichoderma
159
Generally the identification of the Trichoderma spp. usually accepted based on the two DNA
160
gene fragment sequence analysis, while the new Trichoderma spp. can be accepted by at least
161
three DNA barcode fragments analysis [44-46]. Thus present work a total of 18 isolates divided
162
into nine species of Trichoderma were isolated from two different sampling sites of Republic of
163
Korea (Fig.1) and identified based on two DNA gene sequencing analysis including internal
164
transcribed spacer (ITS) and translation elongation factor 1 alpha (tef 1α) based NCBI blast
165
analysis (Fig.2). However, a number of the classification studies have shown that the individual
166
sequence such as ITS, or tef- 1α gene sequences based phylogenic tree was not able to
167
distinguish all Trichoderma spp. Thus combination of multi-loci sequences based phylogenic
168
tree analysis is suggested for better distribution of Trichoderma spp. [47, 48]. Therefore, in the
169
present work was contracted the phylogenetic tree using the concatenated dataset of ITS- tef 1α
170
inferred by maximum parsimony method [49]. The same or closely related species were
171
clustered on a clade on the resulting tree and the test and conference taxa was compared clearly
172
according to earlier report [1, 2, 46, 50, 51]. The present results revealed the similarities between
173
Trichoderma species while the out-group sequence of Nectria berolinensis formed the non-
174
similarity clusters. Interesting the T. harzianum was formed a group of cluster in association with
175
reference sequence while another group was formed for same clades association with other
176
species such as T. virens, T. velutinum and Hypocrea lixii. Similar results were obtained for the 8
177
Viride clades, which indicated the similarity of the species within clades of Trichoderma species.
178
Although, the concatenated dataset of ITS- tef 1α of Trichoderma spp. formed the similar groups
179
according to their species but in case of clades were formed the two different group that's
180
indicated the difference within the clades (Fig.2). For instance, the present study observed two
181
different cluster for Viride and Green/Harzianum from the concatenated dataset of ITS- tef 1α
182
inferred by maximum parsimony tree, which indicated the requirement of further depth
183
molecular assessment for better understanding of the Trichoderma taxonomy. Among the two
184
sites of the coastal area, the site II showed high species diversity and richness (Table.1). The
185
dominant species recorded were T. harzianum. T. atroviride, T. virens, T. velutinum,
186
T.harzianum, T. asperellum, T. koningiopsis, T. aureoviride, and T. koningii (Table 1).
187
3.2. Screening of active biocontrol strains
188
Trichoderma isolates were tested against three phytopathogens (MP, FG and BC) by
189
antagonistic assay. All the strains showed the potential antagonist activity against the targeted
190
pathogens. Among the strains, T. aureoviride (SKCGW013) showed a high inhibition activity
191
against MP (92.5%), FG (94.5%) and BC (89.32%) (Fig.3). Similarly, earlier reports also
192
evidenced the potent inhibitory effect of Trichoderma on pathogens such as Botrytis cinerea[52],
193
Fusarium graminearum [25, 53] and Macrophomina phaseolina [54] through the production of
194
antibiotic metabolites and enzymes mediated competition for nutrients and space[55, 56].
195
Moreover, the strain SKCGW013 was showed the higher enzyme activity such as chitinase
196
(71.21±1.44%), cellulase (68.45±2.32%), protease (48.65±0.12%) and β-(1-3) glucanase
197
(78.15±1.84%) and it was higher than other strains tested in this study. Further study analyzed
198
the metabolites profile of the strain SKCGW013 by applying the chromatography assay. The
199
results showed a total of the 185 secondary metabolites including the polyketides, esters, nitriles, 9
200
alkanes, benzenes, olefins, acids, alcohols and aldehydes in the ethyl acetate extract of
201
SKCGW013 (Fig.4a). Similarly, Trichoderma strains are known to produce chemically
202
diversified antifungal metabolites as the biological weapon against various phytopathogens [57-
203
60]. The antifungal activity of unbounded metabolites of Trichoderma was then tested against
204
fungal pathogen FG. The results showed significant inhibition of FG at the dose depended
205
manner (Fig.4b&c). Similarly the crude extracts of Trichoderma strains are reported to inhibit
206
the growth of F. graminearum and F. oxysporum f. sp. cucumerinum in the PDA plates [8, 25].
207
Thus the present results confirmed the biocontrol potential and stability of unbounded
208
compounds of Trichoderma against phytopathogens.
209
3.3. GC-MS based identification of dominant compounds and computational studies
210
Based on the chromatography, the dominant metabolites from TAE of SKCGW013 were
211
identified as 6-Pentyl-2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept-5-
212
ene-2,3-dicarboxylic acid, 2H-Pyran, 3-bromo-2-butoxytetrahydro-, cis, 2,4-Cyclopentadiene-1-
213
ethanamine,
214
phenylpropinoic acid (Fig.5a). These compounds were selected for the molecular inhibitory
215
interaction towards the proteins - FgSwi6 from the FG [40] and Bcpmr1 from BC [41, 42] by
216
using the computation approach. The docking results showed that all the tested compounds
217
showed good docking score against the targeted proteins, evidencing the synergetic antifungal
218
activity of metabolites from TAE (Table 2). Among the compounds,
219
butoxytetrahydro-, cis (Fig. 5b) displayed higher interaction and inhibitory capacity against the
220
targeted proteins, as indicated by promising docking energy of -8.812 Kcal/mol against FgSwi6
221
and that of -9.808 against Bcpmr1. The active compound 2H-Pyran, 3-bromo-2-
222
butoxytetrahydro-, cis
1,3,3-Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene,
inhibited the expression of 10
and
3-
2H-Pyran, 3-bromo-2-
FgSwi6 by establishing the bond with
223
aliphatic hydrophobic side chain Ile 590, Ile725, Ile 600, Leu593, Ile 368, Ala 724, Leu 362, Ile
224
721, Met 711, Met 677, Val 695 and Ala 676, aromatic hydrophobic side chain Phe 718, and
225
polar neutral side chain Thr 678 (Fig.6a-b). In the case of Bcpmr1, the active compound
226
interacted through bond with aliphatic hydrophobic side chain Leu 436, Leu 435, Leu 396, Ile
227
400, Val 438, and Leu439, and electrically charged side chain Arg 397 (Fig.6c-d). Similar kind
228
of the molecular docking approaches are previously applied to screen the active compounds from
229
Trichoderma against fungal pathogens, such as F. graminearum and F. oxysporum [8, 25]
230
3.4. qRT-PCR Analysis of the secondary metabolites regulatory genes
231
The ketosynthase domain of PKSI gene and adenylation domain of NRPS gene were
232
detected through PCR amplification as these genes are involved in the antimicrobial activity [61].
233
The qRT-PCR results indicated that both genes were expressed but the level of expression was
234
higher in NRPS gene (relative gene expression 2.41) than that in PKS1gene (relative gene
235
expression 9.22). The gene expression indicated the presence of metabolites in TAE belonging
236
to NRPS and PKS1 families that resulted in enhanced antifungal activity [62]. Similarly, the
237
previous results have evidenced the correlation between the expression of the NRPS and PKS1 in
238
the endophytic fungi and their bioactivities including antimicrobial, biomedical and biocontrol
239
activity [63-65].
240
4. Conclusion
241
This work reported the potential of newly isolated T. aureoviride (SKCGW013) on the inhibition
242
of phytopathogens (MP, FG, and BC). The strain synthesised novel metabolites such as 6-Pentyl-
243
2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept-5-ene-2,3-dicarboxylic acid,
244
2H-Pyran,
3-bromo-2-butoxytetrahydro-,
cis, 11
2,4-Cyclopentadiene-1-ethanamine,
1,3,3-
245
Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene, and 3-phenylpropinoic acid as evident
246
by the preliminary metabolism analysis. This calls for critical study on transcriptomes to
247
understand molecular mechanisms adapted by Trichoderma strain for antifungal activity.
248
Therefore, further study will be focused on purification and molecular mechanism of synthesis
249
for the secondary metabolites, produced by T. aureoviride (SKCGW013).
250
Conflict of interest
251
The authors declare that they have no conflict of interest
252
Acknowledgment
253
This work was supported Korea Research Fellowship Program through the National Research
254
Foundation of Korea (NRF) funded by the Ministry of Science, ICT (2017H1D3A1A01052610).
255
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256 257 258 259 260 261 262 263 264 265 266 267 268 269 270 271 272 273 274 275
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Table 1. Description of List of Trichoderma strains collected by this study and their sources Strain code
Culture collection
Identification
Source
KNUP001
NCBI accession ITS1,ITS2 tef-α MG552067 MN513281
CMTCC KNU001
Soil, Wetland forest, Chuncheon
KNUP002
MG552068
MN513282
CMTCC KNU002
SKCGW001
MG552069
MN513283
CMTCC KNU003
SKCGW002
MG552070
MN513284
CMTCC KNU004
SKCGW003
MG552071
MN513285
CMTCC KNU005
SKCGW004
MG940956
MN513286
CMTCC KNU006
SKCGW005
MG940957
MN513287
CMTCC KNU007
SKCGW006
MG940958
MN513288
CMTCC KNU008
SKCGW007
MG940959
MN513289
CMTCC KNU009
SKCGW008
MG940960
MN513290
CMTCC KNU010
SKCGW009
MG940961
MN513291
CMTCC KNU011
SKCGW010
MG940962
MN513292
CMTCC KNU012
SKCGW011
MG940963
MN513293
CMTCC KNU013
SKCGW012
MG940964
MN513294
CMTCC KNU014
Trichoderma atroviride Trichoderma virens Trichoderma velutinum Trichoderma harzianum Trichoderma asperellum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma harzianum Trichoderma koningiopsis Trichoderma koningiopsis Trichoderma
Soil, Wetland forest, Chuncheon Sediemnt, Coastal wetland, Gangwan Sediemnt, Coastal wetland, Gangwan Sediemnt, Coastal wetland, Gangwan Sediemnt, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan
SKCGW013
MG940965
MN513295
CMTCC KNU015
SKCGW014 SKCGW015
MG940966 MG940967
MN513296 MN513297
CMTCC KNU016 CMTCC KNU017
SKCGW016
MG940968
MN513298
CMTCC KNU018
harzianum Trichoderma aureoviride Hypocrea lixii Trichoderma koningiopsis Trichoderma koningii
Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan Sediment, Coastal wetland, Gangwan
Table 2. Interactions between Trichoderma derived compounds and pathogenicity related protein bcpmr1 of Botrytis cinerea and FgSwi6 of Fusarium graminearum. S.no
1 3 5
11.089 24.271
6-Pentyl-2H-pyran-2-one Propionamide
Docking Score (Kcal/mol) Molecular Weight (g/mol) FgSwi6 Bcpmr1 166.22 -8.677 -9.001 73.095 -5.639 -6.192
23.341
2-Aminooctane
129.247
Retention Compound Name time
6 25.554 9 10.382 10 16.287 11
12
17.610 33.302
Bicyclo[2.2.1]hept-5-ene2,3-dicarboxylic acid 182.175 2H-Pyran, 3-bromo-2butoxytetrahydro-, cis 237.13 2,4-Cyclopentadiene-1ethanamine. 109.17 1,3,3-Trimethyl-2(hydroxymethyl)-5-hydroxy1-cyclohexene 170.25 3-phenylpropinoic acid 150.17
-8.356
-9.075
-8.460
-8.344
-8.812
-9. 808
-7.17
-8.485
-8.393 -8.411
-7.683 -9.721
Fig.1. Soil samples collected from two different wetland locations. (i) Soil from wetland forest, Chuncheon si (37°51'19.84"N; 127°44'50.28"E), 2. Sediment from Coastal wetland, Gangwan do (37°24'33.64"N; 129°12'12.89"E) (Sourcehttps://www.google.com/maps/place/Chuncheonsi,+Gangwon-do)
Fig.2. Phylogenetic tree inferred by neighbor joining analysis performed on the ITS-Tef 1α concatenated sequences dataset of Trichoderma spp.
Fig.3. Antagonistic activity of newly isolated Trichoderma strains against three different plant pathogens on PDA (a), percentage of pathogens growth inhibition (b), MP- Macrophomina phaseolina, FG- Fusarium graminearum, BC- Botrytis cinerea.
Fig.4. Distribution of secondary metabolites profile from unbounded extract TAE (a), Antifungal activity of unbounded metabolites derived from Trichoderma sp. (b) and % of inhibition of FG at different concentration of Trichoderma extracts (c).
Fig.5. Chromatography of the potent antifungal compound isolated from T. aureoviride at retention time of 11.089, 24.271, 23.341, 25.554, 10.382, 16.287, 17.610, 33.302 min corresponding to 6-Pentyl-2H-pyran-2-one, Propionamide, 2-Aminooctane, Bicyclo[2.2.1]hept5-ene-2,3-dicarboxylic acid, 2H-Pyran, 3-bromo-2-butoxytetrahydro-, cis, 2,4-Cyclopentadiene1-ethanamine, 1,3,3-Trimethyl-2-(hydroxymethyl)-5-hydroxy-1-cyclohexene, and 3phenylpropinoic acid (a), the potent antifungal compound structure of 2H-Pyran, 3-bromo-2butoxytetrahydro-, cis, (b)
Fig.6. 3D and 2D structure demonstrate the interaction between 2H-Pyran, 3-bromo-2butoxytetrahydro-, cis with FgSwi6 from filamentous fungus Fusarium graminearum (a, b) and Bcpmr1 from B. cinera (c,d).
Highlights • This work reported the potent biocontrol strain from wetland soil of Republic of Korea. • A total of nine Trichoderma species was isolated with potent biocontrol properties • T. auroviride (SKCGW013) inhibited the growth of various phytopathogens • Metabolites from the T. auroviride induced biocontrol activity synergistically
Declaration of interests ☐ The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper.