Tri11, tri3, and tri4 genes are required for trichodermin biosynthesis of Trichoderma brevicompactum.

Trichoderma brevicompactum and T. arundinaceum both can synthesize trichodermin with strong antifungal activity and high biotechnological value. The two Trichoderma species have a tri cluster, which includes seven genes (tri14, tri12, tri11, tri10, tri3, tri4, and tri6) that encode transport and regulatory enzymes required for the biosynthesis of trichodermin. Here, we isolated T. brevicompactum 0248 transformants with disrupted tri11, tri4, or tri3 gene. We also described the effect of tri11, tri3, or tri4 deletion on the expression of other genes in the tri cluster. Targeted Δtri3 knockout mutant exhibited a sharp decline in the production of trichodermin, and trichodermol, which is a substrate for trichodermin production, accumulated. Thus, the results demonstrated that tri3 was responsible for the biosynthesis of trichodermin, and the tri3 gene-encoded enzyme catalyzed the acetylation reaction of the hydroxy group at C-4 of the trichodermin skeleton. In addition, tri4 and tri11 deletion mutants were generated to evaluate the roles of tri4 and tri11 in trichodermin biosynthesis, respectively. Deletion mutant strain Δtri4 or Δtri11 did not produce trichodermin in T. brevicompactum, indicating that tri4 and tri11 are essential for trichodermin biosynthesis. This is the first to report the function of tri3, tri4 and tri11 in T. brevicompactum, although the role of tri4 and tri11 has already been described for T. arundinaceum by Cardoza et al. (Appl Environ Microbiol 77:4867-4877, 2011).

Introduction

Trichoderma species are well-known biological control agents of diseases in numerous crops, and these species produce many antifungal compounds and cell-wall-degrading enzymes (Harman 2006; Malmierca et al. 2012; Tijerino et al. 2011a, b). The biocontrol activities of Trichoderma spp. against phytopathogenic fungi generally include antibiosis, parasitism, and competition for space and nutrients (Harman 2006). Antibiotic molecules synthesized by Trichoderma are low-molecular-weight and volatile metabolites as well as high-molecular weight polar metabolites. The former type includes simple aromatic compounds, polyketides, volatile terpenes, and isocyanide metabolites, while the latter includes peptaibols and diketopiperazine-like gliotoxin and gliovirin compounds (Reino et al. 2008; Szekeres et al. 2005; Tijerino et al. 2011a). Trichothecenes belong to a large group of terpenoid-derived secondary metabolites and are mainly synthesized by Fusarium and other fungal genera, such as Trichoderma, Myrothecium, Spicellum, Stachybotrys, and Trichothecium (Shentu et al. 2014a; Wilkins et al. 2003). Terpenes are derived from the repetitive fusion of branched five-carbon units based on an isopentane skeleton, and most of the chemical intermediates in their biosynthetic pathway have been identified (Tijerino et al. 2011b). The trichothecene biosynthetic pathway in Fusarium has been documented and extensively reviewed (Kimura et al. 2007). However, the genes involved in trichothecene biosynthesis in the other genera remain unknown.

Trichodermin and harzianum A (HA), which are synthesized by T. brevicompactum and T. arundinaceum, belong to terpenes and have similar structures except for the side chain group at C-4 (an acetyl group and an octa-2,4,6-trienedioic acid, respectively) (Malmierca et al. 2012). T. arundinaceum has been used as a model to study the beneficial effect of trichothecenes on the Trichoderma biocontrol activity and modulation of plant defense responses of this fungus (Malmierca et al. 2012). Furthermore, bioactivity assays have shown that trichodermin synthesized by T. brevicompactum exhibits stronger antifungal activity against Saccharomyces cerevisiae, Kluyveromyces marxianus, Candida albicans, Aspergillus fumigatus, Botrytis cinereal, and Rhizoctonia solani than amphotericin B and hygromycin (Shentu et al. 2014a; Tijerino et al. 2011a). The mechanism and genes involved in the trichothecene biosynthesis in Trichoderma have been increasingly investigated. Although Fusarium and Trichoderma can synthesize trichothecenes, these species have remarkably different organizations of genes in the tri cluster and trichothecenes biosynthesis (Cardoza et al. 2011). TRI gene orthologues (tri) in T. arundinaceum and T. brevicompactum had been identified and characterized. The result showed that both Trichoderma species have a tri cluster with seven homologous genes in the Fusarium TRI cluster (Cardoza et al. 2011). Furthermore, the two Trichoderma species have the same organizations of genes in the tri cluster but different from that in Fusarium (Cardoza et al. 2011). Sequence and functional analyses demonstrated that the gene (tri5) responsible for the first step in trichothecene biosynthesis is located outside the cluster in both Trichoderma species but inside the cluster in Fusarium (Cardoza et al. 2011). Thus, analysis of the heterologous gene expression indicates that the two T. arundinaceum cluster genes (tri4 and tri11) differ in function from their Fusarium orthologues (Cardoza et al. 2011). The Tatri4-encoded enzyme catalyzes only three of the four oxygenation reactions catalyzed by the orthologous enzyme in Fusarium (Cardoza et al. 2011). By contrast, the Tatri4-encoded enzyme in T. arundinaceum has the same function as that of MrTri4-encoded enzyme in Myrothecium (McCormick and Alexander 2007). The Tatri11-encoded enzyme catalyzes a reaction (trichothecene C-4 hydroxylation) that is completely different from that of the Fusarium orthologue (trichothecene C-15 hydroxylation) (Cardoza et al. 2011). However, the function of tri3 gene in T. arundinaceum remains ambiguous. The lateral moiety at the C-4 position of the HA might be added to trichodermol through acetylation using an acyltransferase encoded by the tri3 gene (Cardoza et al. 2011). The tri5 gene has a significant role in the production of trichodermin in T. brevicompactum such that its overexpression increases trichodermin production and antimicrobial activity (Tijerino et al.2011a, b). However, whether tri3 participates in the trichodermin biosynthesis remains unknown. The functions of tri11 and tri4 in T. brevicompactum should be verified. These genes are orthologues with Tatri11 and Tatri4 of T. arundinaceum.

We have identified and characterized the tri cluster of T. brevicompactum 0248, which can biosynthesize trichodermin (Yuan et al. 2016). The results indicated that T. brevicompactum 0248 has a 24,793 bp cluster that includes tri14, tri12, tri11, tri10, tri3, tri4, and tri6 genes which are highly homologous to those in the T. arundinaceum tri cluster (Yuan et al. 2016). Furthermore, the tri cluster in strain 0248 is highly homologous to that of the reported strain T. brevicompactum IBT 40841. Strain 0248 and IBT 40841 clusters primarily differ in the size of the tri11–tri12 intergenic region, which is 2287 bp in strain 0248 and 3000 bp in IBT 40841. In this study, we described the effects of the disruption of tri11, tri3, and tri4 in T. brevicompactum 0248 on trichodermin production and gene expression of the other tri genes in trichodermin biosynthesis.

Materials and methods

Strains, culture media, and culture conditions

Trichoderma brevicompactum 0248 was isolated in our previous study and deposited in the China General Microbiological Culture Collection Center (CGMCC 6985) (Shentu et al. 2014b). The isolate was maintained on a potato-dextrose agar (PDA) slant medium at 4 °C until used.

Agrobacterium tumefaciens AGL-1, which was obtained from the Zhejiang Provincial Key Laboratory of Biometrology and Inspection and Quarantine, was grown in YEB medium with 100 µg/mL rifampicin at 28 °C before use for A. tumefaciens-mediated transformation (ATMT) (Lacorte et al. 1991). The tri11, tri3, and tri4 genes in the tri cluster of T. brevicompactum 0248 were deleted by homologous recombination method as previously described (Brown et al. 2004; Kumar 2010).

The plasmid pSilent-1, which was provided by the Fungal Genetics Stock Center in USA, carried a hygromycin-resistant gene (hph) cassette. The plasmid pCAMBIA0380, which was obtained from the Zhejiang Provincial Key Laboratory of Biometrology and Inspection and Quarantine, was used for ATMT.

All primers were synthesized by Shanghai Sunny Biotechnology Co. Ltd and are listed in Additional file 1: Table S1, Additional file 2: Table S2, Additional file 3: Table S3.

Construction of recombinant vector

First, using plasmid pSilent-1 as template, hph was amplified by PCR with primers Ph-F/Ph-R (Additional file 1: Table S1) to obtain the hph expression cassette. Then, 1-kb upstream DNA fragment before the tri11, tri3, and tir4 gene start codon was amplified using total DNA as template and corresponding primers P11-5F/P11-5R, P3-5F/P3-5R, and P4-5F/P4-5R. The forward primers P11-5F, P3-5F, and P4-5F contained the BstXI site, while the reverse primers P11-5R, P3-5R, and P4-5R contained a 22 bp reverse complementary sequence of the hph cassette. Similarly, another DNA fragment downstream of the tri11, tri3, and tir4 gene stop codon was amplified using primers P11-3F/P11-3R, P3-3F/P3-3R, and P4-3F/P4-3R, respectively. The forward primers P11-3F, P3-3F, and P4-3F contained a 22 bp overlapping sequence of the hph gene, while the reverse primers P11-3R, P3-3R, and P4-3R contained an XmaI site (Fig. 1). Then, the above three linearized fragments were equimolarly mixed and cycled in a fusion PCR to generate a gene knockout fragment (Cao et al. 2014). The corresponding gene knockout fragments were cloned into the BstXI/XmaI sites of pCAMBIA0380 to generate the corresponding expression constructs designated as pKT11, pKT3, and pKT4 (Fig. 1).

Fig. 1

Construction of the recombinant plasmid for gene knockout. First, using plasmid pSilent-1 as the template, hygromycin resistance gene was amplified by PCR. An approximately 1-kb upstream DNA fragment before the tri3, tri4, and tir11 gene start codon and another 1-kb upstream DNA fragment downstream of the tri3, tri4, and tir11 gene stop codon were amplified to obtain homology L and R, respectively. Second, the above three linearized fragments were equimolarly mixed and cycled in a fusion PCR to generate a gene knockout fragment. Third, the corresponding gene knockout fragments were cloned into the BstXI/XmaI sites of pCAMBIA0380 to generate the corresponding vectors designated as pKT3, pKT4, and pKT11

Transformation of T. brevicompactum 0248

The expression vectors pKT11, pKT3, and pKT4 were transformed using ATMT as described previously (Dos et al. 2004; Yang et al. 2011). The obtained transformants were confirmed by PCR and subcultured in PDA plates with 100 µg/mL hygromycin B for three generations to test the genetic stability.

Quantitative RT-PCR (QRT-PCR) analysis

Total RNA of T. brevicompactum 0248 and Δtri11, Δtri3, and Δtri4 knockout strains were isolated using Spin Column Fungal Total RNA Purification Kit (Sangon, Shanghai, China). The total cDNA was obtained through reverse-transcription reaction using PrimeScript® RT Reagent Kit with gDNA Eraser (TaKaRa, Dalian, China). QRT-PCR was performed in an Applied Biosystems StepOnePlus Real-Time PCR System using a SYBR® Premix Ex TaqTM (TliRHaseH Plus) reagent (TaKaRa, Dalian, China) (Shentu et al. 2014a). The primers used in qRT-PCR are listed in Additional file 2: Table S2. The acceptable qRT-PCR standard curve (0.95 ≤ E ≤ 1.05, R2 ≥ 0.99) of the gene examined in this study was optimized by varying the annealing temperature and annealing time. The β-tubulin gene of T. brevicompactum 0248 was used as the reference gene (Shentu et al. 2014a). Quantification of the relative gene expression was analyzed by the 2−ΔΔCt method.

Analysis of trichodermin using gas chromatography (GC)

The fermentation broth was separated from the mycelia by filtration using a Buchner funnel and extracted exhaustively with ethyl acetate (v/v, 1:2). The organic fractions were combined and evaporated to dryness in a vacuum at 50 °C. The recovered residues were resuspended in methanol and analyzed using GC to quantify trichodermin (Shentu et al. 2008).

Results

Isolation of tri11, tri3, and tri4 deletion mutants

Using the gene-deletion plasmid and ATMT, transformants were selected on PDA plates with 100 µg/mL hygromycin B. Then, these transformants were further identified by PCR using the primers P11N-R/P11N-F, P3N-R/P3N-F, and P4N-R/P4N-F (Additional file 3: Table S3) to verify Δtri11, Δtri3, and Δtri4 mutants, respectively. Figure 2a shows that 10 transformants were arbitrarily chosen for PCR analysis, of which transformants 2, 5, 6, and 10 (lanes 2, 5, 6, and 10, respectively) did not exhibit the expected 1.1 kb band. Furthermore, primer pair P3W-R/P3W-F was designed according to the flanking sequence of the upstream/downstream DNA fragments of tri3. This pair was used to verify whether transformants 2, 5, 6, and 10 had the expected 3.6 kb band. The length of the hph cassette and ORF of the tri3 were 1.1 and 1.78 kb, respectively. The band of lane 22 from the fragment of the wild strain was 4.3 kb. If the ORF of the tri3 was replaced successfully by the hph cassette in mutants, transformants 2, 5, 6, and 10 (lanes 13, 16, 17, and 21, respectively) should show the expected 3.6 kb band (reduced by approximately 0.7 kb). These expected results were observed (Fig. 2a), indicating that Δtri3 mutants were obtained successfully. Δtri11 and Δtri4 mutants were verified with the same method (Figs. 2b and c). Four transformants (lanes 1, 4, 5, and 7) in which the hph cassette replaced the ORF of the tri11 gene were identified (Fig. 2b). Five transformants (lanes 3, 4, 6, 8, and 9) in which the hph cassette replaced the ORF of the tri4 gene were also determined (Fig. 2c).

Fig. 2

Agar gel analysis. a Verification of tri3 deletion. Numbers from 1 to 10 and 12 to 21 refer to the arbitrarily chosen transformants. Numbers 11 and 22 refer to the wild strain. The numbers and their corresponding transformants are as follows: 1 and 12, Δtri3-1; 2 and 13, Δtri3-2; 3 and 14, Δtri3-3; 4 and 15, Δtri3-4; 5 and 16, Δtri3-5; 6 and 17, Δtri3-6; 7 and 18, Δtri3-7; 8 and 19, Δtri3-8; 9 and 20, Δtri3-9; and 10 and 21, Δtri3-10. Lanes 2, 5, 6, and 10 did not show the expected band of 1.1 kb. This result indicated that tri 3 was deleted in Δtri3-2, Δtri3-5, Δtri3-6, and Δtri3-10, respectively. Furthermore, Δtri3-2, Δtri3-5, Δtri3-6, and Δtri3-10 (lanes 13, 16, 17, and 21, respectively) showed the expected band of 3.6 kb (reduced by approximately 0.7 kb). The ORF of the tri3 was replaced successfully by the hygromycin cassette in these mutants. b Verification of tri11 deletion. Numbers from 1 to 9 and 11 to 19 refer to the arbitrarily chosen transformants, while numbers 10 and 20 refer to the wild strain. The numbers and their corresponding transformants are as follows: 1 and 11, Δtri11-1; 2 and 12, Δtri11-2; 3 and 13, Δtri11-3; 4 and 14, Δtri11-4; 5 and 15, Δtri11-5; 6 and 16, Δtri11-6; 7 and 17, Δtri11-7; 8 and 18, Δtri11-8; and 9 and 19, Δtri11-9. Lanes 1, 4, 5, and 7 did not show the expected band of 1.1 kb. This result indicated that tri11 was deleted in Δtri11-1, Δtri11-4, Δtri11-5, and Δtri11-7, respectively. Furthermore, Δtri11-1, Δtri11-4, Δtri11-5, and Δtri11-7 (lanes 11, 14, 15, and 17, respectively) showed the expected band of 3.6 kb (reduced by approximately 0.7 kb). The ORF of the tri11 was replaced successfully by the hygromycin cassette in these mutants. c Verification of tri4 deletion. Numbers from 1 to 9 and 11 to 19 refer to the arbitrarily chosen transformants, while numbers 10 and 20 refer to the wild strain. The numbers and their corresponding mutants are as follows: 1 and 11, Δtri4-1; 2 and 12, Δtri4-2; 3 and 13, Δtri4-3; 4 and 14, Δtri4-4; 5 and 15, Δtri4-5; 6 and 16, Δtri4-6; 7 and 17, Δtri4-7; 8 and 18, Δtri4-8; and 9 and 19, Δtri4-9. Lanes 3, 4, 6, 8, and 9 did not show the expected band of 1.1 kb. This result indicated that tri4 was deleted in Δtri4-3, Δtri4-4, Δtri4-6, Δtri4-8, and Δtri4-9, respectively. Furthermore, Δtri4-3, Δtri4-4, Δtri4-6, Δtri4-8, and Δtri4-9 (lanes 13, 14, 16, 18, and 19, respectively) showed the expected band of 3.6 kb (reduced by approximately 0.7 kb). The ORF of the tri4 was replaced successfully by the hygromycin cassette in these mutants

Effect of tri3 deletion on the expression of the tri genes

The relative expression levels of the tri genes in the Δtri3 mutant were analyzed and compared with those of the wild-strain 0248. The expression of the tri3 gene in the wild strain changed with culture time (16, 28, 40, 52, 64, 76, and 88 h), with the highest expression level observed at fermentation for 40 h (Fig. 3a). The tri3 expression was not detected in the Δtri3 mutant at each time point. Surprisingly, the deletion of tri3 resulted in the significant upregulation of the expression of tri4, tri5, tri6, tri10, tri11, tri12, and tri14 genes compared with that of the wild type after 40 h of culture. The expression of these genes in Δtri3 mutant had remarkably declined from 52 to 88 h (Fig. 3).

Fig. 3

Expression of tri genes in Δtri3 mutant and wild strain. The quantification of tri3 gene expression in the different culture times was analyzed by 2−ΔΔCt method. The wild strain cultured for 88 h was used as control and β-tubulin as reference gene. a tri3, b tri4, c tri5, d tri6, e tri10, f-tri11, g tri12, and h tri14

Effect of tri4 deletion on the expression of the tri genes

We determined whether the deletion of tri4 gene affected the transcription of tri genes. The relative expression levels of tri3, tri4, tri5, tri6, tri10, tri11, tri12, and tri14 in the Δtri4 mutant and wild strain 0248 were detected. The tri4 expression was not detected in the Δtri4 mutant at each time point (Fig. 4). The deletion of tri4 positively affected the expression of tri3, tri5, tri6, tri10, tri11, tri12, and tri14 compared with the wild-type strain at 40 h. After 52 h of fermentation, the expression levels of these genes declined.

Fig. 4

Expression of tri genes in Δtri4 mutant and wild strain. The quantification of tri4 gene expression in the different culture times was analyzed by 2−ΔΔCt method. The wild strain cultured for 88 h was used as control and β-tubulin as reference gene. a tri3, b tri4, c tri5, d tri6, e tri10, f tri11, g tri12, and h tri14

Effect of tri11 deletion on expression of the tri genes

The tri11 deletion process was successful, and no expression of tri11 was found in the Δtri11 mutant. After 52 h of culture, the expression level of tri3 was higher in the Δtri11 mutant than in the wild strain. At other time points, relative expression levels of tri3, tri4, tri5, tri6, tri10, tri12, and tri14 in the Δtri11 mutant were higher than in the wild strain (Fig. 5).

Fig. 5

Expression of tri genes in Δtri11 mutant and wild strain. The quantification of tri11 gene expression in the different culture times was analyzed by 2−ΔΔCt method. The wild strain cultured for 88 h was used as control and β-tubulin as reference gene. a tri3, b tri4, c tri5, d tri6, e tri10, f tri11, g tri12, and h tri14

Effect of tri3, tri4, or tri11 deletion on trichodermin production

Given that trichodermin is the sole product of the tri cluster in T. brevicompactum 0248, the concentrations of trichodermin in the culture extracts were analyzed by GC in both wild strain and Δtri gene mutants. No trichodermin was detected in the Δtri4 and Δtri11 mutants. That is, tri4 or tri11 deletion directly affected trichodermin biosynthesis by T. brevicompactum. However, Δtri3 mutant could still biosynthesize trichodermin, although tri3 gene was deleted (Fig. 6a). Prolonged cultivation time resulted in increased trichodermin concentration in the Δtri3 mutant and strain 0248, although the trichodermin yield by Δtri3 mutant was lower than that of the wild strain at 76 h of fermentation by approximately 40 mg/L trichodermin. Deletion of tri3 gene resulted in reduced trichodermin content. Furthermore, high abundance of trichodermol in the Δtri3 strain was detected after 40 h cultivation, contrary to the quite low trichodermol content in the wild-type culture extracts (Fig. 6b). It was shown that trichodermol was accumulated in the culture broth of Δtri3 mutant.

Fig. 6

a Trichodermin production by Δtri3 mutants and wild strain 0248. b Trichodermol production by Δtri3 mutants and wild strain 0248

Discussion

Trichoderma is an interesting fungus because of its important application in biocontrol (Malmierca et al. 2012). However, T. brevicompactum has not been well-studied among Trichoderma, because T. brevicompactum (IBT 9471) had been erroneously considered as T. harzianum (ATCC 90237) because of substantial shared micromorphology of these two species (Nielsen et al. 2005; Degenkolb et al. 2008). Until 2005, this IBT 9471 strain has been reclassified as T. brevicompactum on the basis of phylogenetic lineage within the morphological species T. brevicompactum and trichothecene production (Nielsen et al. 2005; Shentu et al. 2014a). Previous studies reported that T. brevicompactum is one of the Trichoderma species that produces trichodermin, which exhibits strong antifungal activity and has high biotechnological value (Tijerino et al. 2011a, b). Therefore, conducting systematic studies on this species is necessary and urgent.

In this study, tri4 and tri11 deletion mutants were generated to evaluate the roles of tri4 and tri11 in trichodermin biosynthesis. Tatri4 catalyzes the addition of oxygen at C-2, C-12, and C-11, and this process converts trichodiene to isotrichodiol in T. arundinaceum. Deletion mutant strain Δtri4 did not produce trichodermin in strain 0248, and this phenomenon was previously observed for T. arundinaceum Δtri4 mutants (Cardoza et al. 2011; Malmierca et al. 2012). This result suggested that tri4 is essential for trichodermin biosynthesis in T. brevicompactum. Tatri11 controls the hydroxylation at C-4, and this process converts 12,13-epoxytrichothec-9-ene (EPT) to trichodermol in T. arundinaceum. Deletion mutant strain Δtri11 also did not biosynthesize trichodermin in T. brevicompactum 0248. Thus, these results first proved the necessity of tri11 for trichodermin biosynthesis in T. brevicompactum.

In T. arundinaceum, Tri3 is hypothesized to acetylate oxygen at C-4 of the trichothecene skeleton based on the amino acid sequence and motif, HXXXDG, which is indicative of acetyl-transferases (Murray and Shaw 1997). However, the function of tri3 in Trichoderma has not been verified yet. In our study, Δtri3 deletion mutant strain was obtained. The trichodermin in Δtri3 cultures was detected using GC, and the results showed lower concentration in the Δtri3 deletion mutant than in the wild type. As expected, the tri3 gene was involved in the biosynthesis of trichodermin by T. brevicompactum. Furthermore, high abundance of trichodermol in the Δtri3 strain was detected, contrary to the quite low trichodermol content in the wild-type culture extracts. These results demonstrated that deletion of tri3 gene in T. brevicompactum 0248 reduced the trichodermin content and accumulated trichodermol. Thus, tri3 gene was responsible for the acetyl moiety to the C-4 oxygen in T. brevicompactum.

Small amount of trichodermin was still detected in the Δtri3 mutants. This phenomenon was also observed for deletion mutants of Fusarium sporotrichioides (McCormick et al. 1996; Garvey et al. 2009). Trace amounts of trichothecene T-2 toxin were detected in tri3 mutants of F. sporotrichioides (McCormick et al. 1996). The small amount of trichodermin suggested the presence of another acetyl-transferase that can convert trichodermol into trichodermin but with lower efficiency. This result implied that an unidentified enzyme analogous to the tri3 acetylase from T. brevicompactum strain was probably responsible for the catalysis of the C-4 hydroxyl group of trichodermol. Many unigenes homologous to the acyltransferase-encoding genes were found in our previous transcriptome analysis of T. brevicompactum 0248 (Shentu et al. 2014a). In summary, our results indicated that tri3 gene was responsible for the last step of the acetylation of the C-4 oxygen in T. brevicompactum.

Interestingly, QRT-PCR analyses showed that before 52 h cultivation, the loss of function of tri3, tri4, or tri11 led to the upregulation of the tri genes. These results were in agreement with the feedback regulation mechanism. To our knowledge, the end-product and intermediate metabolites play a significant role in the regulation of metabolic pathways by directly or indirectly regulating the genes involved in metabolic pathways (Goelzer et al. 2008; Herrgard et al. 2006). Previous studies showed that the synthesis of trichodermin was mainly concentrated during the incubation period of 40–60 h (Yuan et al. 2016). Therefore, the lower yield of trichodermin in Δtri3 mutant or intermediate metabolites in Δtri4 and Δtri11 mutants may serve as a signal to trigger the feedback regulation. Thus, the expression of tri genes was upregulated, and synthesis of enzymes was induced.

In conclusion, T. brevicompactum is an important species because of its high biocontrol potential. The biosynthesis of trichothecenes by T. brevicompactum has been elucidated. It is first proved that tri4 and tri11 are essential for trichodermin biosynthesis by T. brevicompactum. This study is also the first to report the function of tri3 in Trichoderma, and the results confirmed the previous hypothesis on the tri3 function in the biosynthesis of trichothecenes.

Additional file 1: Table S1. Primers used to construct plasmid pKT.

Additional file 2: Table S2. Primers used for qRT-PCR.

Additional file 3: Table S3. Primers used to verify transformants.