Regulatory Effects of Nitric Oxide on Reproduction and Melanin Biosynthesis in Onion Pathogenic Fungus Stemphylium Eturmiunum

The formation of propagules (conidia and ascospores) is the critical stage for the transmission of the pathogenic fungus Stemphylium eturmiunum. However, how the development of these propagules is regulated remains to be fully understood. Here, we show that nitric oxide (NO) is necessary for the formation of conidia and pseudothecia in S. eturmiunum. Application of NO scavenger carboxy-CPTIO (cPTIO) or soluble guanylate cyclase (sGC) inhibitor NS2028 abolishes the formation of conidia and pseudothecia. In the culture of S. eturmiunum, supplement of NO-releasing compound sodium nitroprusside (SNP) results in an increased formation of conidia at 0.2 mmol/L, and pseudothecia at 2 mmol/L. SNP supplement also triggered increased biosynthesis of melanin, which can be inhibited partially upon the addition of either arbutin or tricyclazole, the specic inhibitors for 3,4-dihydroxyphenylalanine (DOPA) and dihydroxynaphthalene (DHN) synthetic pathway, respectively. Intriguingly, enhanced melanin biosynthesis triggered an increased formation of propagules; while its inhibition impaired their formation. The SNP-induced increment in the formation of propagules can be also compromised upon supplement of cPTIO or NS-2028. RT-PCR analysis showed that SNP at 0.2 mmol/L promoted transcription of the genes encoding the conidiation co-regulators brlA, abA, and wetA, and inhibited at 2 mmol/L. In contrast, application of SNP at 2 mmol/L increased transcription of the genes encoding mat1, and mat2, the genes related to sexual reproduction, and the transcription of two DNH melanin synthetic genes pks1 and pks2, and the key gene tyr for DOPA melanin biosynthesis. However, the increased transcription of these genes is down-regulated or blocked upon supplement of cPTIO or NS-2028. Thus, NO regulates asexual and sexual development, as well as melanin synthesis in S. eturmiunum possibly through NO-sGC-GMP signaling pathway.


Introduction
The foliar fungal pathogen Stemphylium eturmiunum is a homothallic lamentous ascomycete causing severe leaf blight of onions (Fernandez and Rivera-vargas 2008). In addition, S. eturmiunum is also a postharvest spoiler of fresh tomatoes (Andersen and Frisvad 2004;Trinetta et al. 2013). The infection at the lesions of fresh tomatoes by the fungus results in the production of toxic metabolites infectopyrone and macrosporin (Andersen and Frisvad 2004). In natural habitats, S. eturmiunum develops asexual conidiophores for conidiation, and sexual fruiting bodies pseudothecia for producing ascospore (Simmons 2001). The conidia that easily reach the host alveola are the major infective propagules  (Engh et al. 2007). Similar to conidia, the unique structure of pseudothecia also confers fungi the capacity to survive in harsh environment (Lambou et al. 2008;Zhao et al. 2017). Thus, the involvements of melanin in the construction of conidia and pseudothecia endow the resistance of fungi against environmental insults and the effective infection and transmission (Pal et al. 2014).
Asexual sporulation is the most common mode for reproduction and transmission in lamentous fungi ) and is timed and genetically programmed (Adams et al. 1998; Lee et al. 2010). In Aspergillus, the conidial sporulation is determined by a central regulatory pathway, where the transcriptional factors brlA, abaA, wetA coordinate conidiation-speci c gene expression and determines the order of gene activation during the formation of conidiophores and maturation of conidia (Boylan et a., 1987;Mirabito et al. 1989).
Similar to asexual sporulation, the formation of pseudothecia is also regulated by multiple genes.
Previously, we showed that the development of pseudothecia in S. eturmiunum is regulated not only by the genes encoding MAT1, MAT2, and the protein in G-protein signaling pathway but also by magl, the gene responsible for the synthesis of arachidonic acid (Zhao et al. 2019). Treatment of S. eturmiunum with 5-azacytidine (5-AC) resulted in the complete silence of magl followed by disruption in the development of pseudothecia and melanin synthesis. Interestingly, the impaired development of In lamentous fungi, the communication with habitats is achieved by complex signaling systems that determine the fungal proliferation, development, and in some cases virulence (Kozubowski et al. 2009). The well-known signaling pathways in fungi include the protein kinase A/cyclic AMP (cAMP), protein kinase G/cyclic GMP (cGMP), protein kinase C (PKC)/mitogenactivated protein kinase (MAPK), lipid signaling cascades, and the calcium-calcineurin signaling pathway (Kozubowski et al. 2009). PKG/cGMP pathway, which seems to exist in lamentous fungi, is activated by free radical molecule NO (Zhao et al. 2020). The NO, highly diffusible within the cell or through cell membrane (Lancaster 1997), can work as a transient, local, intra-or intercellular signaling molecule in miscellaneous biological systems including fungi (Culotta and Koshland 1992). In fungi, NO signaling is involved in conidiation, formation of sexual fruiting bodies, and regulation of secondary metabolism (Zhao et al. 2020). Established evidences have shown that NO can function as the activator of sGC able to bind selectively with the hemoprotein in sGC even in the presence of oxygen (Boon and Marletta 2005). The binding of NO with Heme iron triggers the change sGC conformation and subsequently activates its catalytic domain, where GTP can be catalyzed to cyclic GMP (cGMP) (Friebe and Koesling 2003). The produced cGMP then combines with PKG, which constitutes central downstream mediator of NO-cGMP-PKG signaling pathway, and orchestrates pathway-speci c cellular response through the phosphorylation of phosphorylation-dependent transcriptional factors (Contestabile 2008).
Studies in the past decades have shown that NO-mediated signaling networks are involved in conidiation (Wang and Higgins 2005;Gong et al. 2007), the formation of parasitic structure of appressoria (Prats et al. 2008), asexual structures of sporangiophores (Maier et al. 2001), and sexual structures of cleistothecia in Aspergillus species (Baidya et al. 2011). In our previous attempts to unravel the regulatory mechanisms for sexual development of S. eturmiunum, we found that treatment of the fungus with 5-AC resulted in the formation albinism phenotype and the silence of the genes responsible for melanins synthesis in addition to magl. Application of SNP partially restored biosynthesis of melanins in 5-AC treated S. eturmiunum. Intriguingly, SNP supplement in non-treated S. eturmiunum increased the number of conidia and pseudothecia. However, how NO signaling affects asexual and sexual development remains to be established. In this study, we used SNP as the external NO source to probe the regulatory effects of NO on conidiation, sexual fruiting body formation, and production of melanin. Our data showed that NO-induced increment in conidiation, formation of pseudothecia, and melanin accumulation is possibly mediated by NO-cGMP signaling pathway, where NO works as a sGC activator triggering the signal transduction cascade.

Gene transcription analysis
For RNA extraction, the mycelia were grounded with pestle and mortar in liquid nitrogen followed by extraction using Trizol (Takara, Ishiyama, Japan) as previously described (Lee et al. 1997). cDNA was generated using the Prime Script™ RT reagent kit (Takara, Ishiyama, Japan). Gene transcription analysis was conducted by quantitative real-time PCR (RT-PCR). The forward (F) and reverse (R) oligonucleotide primer sequences were listed in Table 1. RT-PCR was carried out using the Fast SYBR Green Master Mix (Thermo Fisher Scienti c, USA). Gene expression levels were normalized using the endogenous control gene actin. To characterize the changes of mRNA levels of the genes in uenced by NO, we employed Ct value of the initial amount of the candidate mRNA in a sample, as a quantitative measurement of gene expression strength under speci c experimental conditions and simultaneously performed RT-PCR of the genes in the samples treated and untreated by SNP followed by double △Ct analysis. The relative mRNA level was indicated by the exponentiation of 2 −△△Ct (Livak and Schmittgen 2001). Every experiment was independently performed three times.

Assay of NO levels and NO producing capacity activity
For assaying NO levels and NO producing capacity, the mycelia were withdrawn and rinsed twice with pure water and disrupted with mortar and pestle in liquid nitrogen. The well-powdered mycelia were then used for the assay of NO production and NO producing capacity. NO levels were determined by total NO assay kit (A012-1-2, Nanjing Jiancheng Bioengineering Institute, China), and its levels were indicated as micromolar per milligram protein (µmol/mg prot). NO producing capacity in homogenates was estimated using a total NOS assay kit (A014-2-1, Nanjing Jiancheng Bioengineering Institute, China). The protein content was determined by Coomassie Brilliant Blue using BSA (High-Tech Innovation, Inc., Shanghai, China) as standard. NO producing capacity was demonstrated as units (U). One unit of NO producing capacity stands for the number of micromoles of NO produced by 1 mg protein in 1 min (Zhao et al. 2015). Each experiment was independently performed at least three times.

Pathways for melanin biosynthesis
The pathway for melanin synthesis was determined by the application of speci c pathway inhibitors. were inoculated by placing a mycelium plug cut from the margins of an actively growing colony, and incubated at 26 °C for 7d followed by observation of growth and pigmentation. Every experiment was independently performed three times.

Tyrosinase activity
Tyrosinase activity was assayed as described (Lejczak et al. 1987

Melanin extraction
Melanin extraction from the fungal biomass was performed as described previously (Pal et al. 2014) with a slight modi cation. In brief, the mycelia were crushed with 2 mol/L NaOH (pH 10.5) and placed for 48 h.
Next, the mixture was centrifuged at 3500 g for 15 min and the resultant supernatant was mixed with 6 mL of a mixture solvent consisting of chloroform, ethyl acetate and ethanol (2 mL each), and vortexed for 5 min at room temperature to remove lipids. After removal of the organic layer, the aqueous layer was acidi ed by 2 mol/L HCl to pH 2.5 followed by incubation overnight at room temperature and then centrifuged at 3500 g for 15 min to remove carbohydrates and proteins. The resultant precipitate was dried at room temperature, and dissolved in 2 mol/L NaOH followed by centrifugation at 3500 g for 15 min. The supernatant was then acidi ed with 6 mol/L HCl. And centrifuged at 3500 g for 15 min. The resultant precipitate was washed with distilled water and dried at room temperature, and used until further analysis.
Heterologous expression of the genes involved in biosynthesis of DHN melanin A. nidulans LO8030 (Chiang et al. 2013) was used as heterologous host to express the genes involved in DHN melanin biosynthesis. For constructing the heterologous transformants, one 1.5 Kb up-and downstream of the two pks genes were fused with pyrG by fusion PCR using the primers listed in Table 1.
The fused DNA fragments were then transformed to wA locus in A. nidulans LO8030 following the protocol described previously (Brock et al. 2008). All constructions were con rmed by diagnostic PCR.

Protection of conidial germination under UV irradiation
The conidia were irradiated by UV (30 W) at a distance of 65 cm for 15 min. After exposure to UV, the conidia were suspended in 20% Tween 80 and reconstituted to a nal concentration of 500 cfu/mL using a hemocytometer. A total of 200 µL was pipetted to plate spreading on GMM agar media. For germination assay, the conidia-spread plates were incubated at 37 °C for 24 h. The germination rate was calculated by the number of germinated conidia divided by the number of conidia in 200 µL conidia suspension.

Statistical analysis
All determinations were carried out in triplicate and the results are expressed as mean ± standard deviation (SD). Excel was used to compare the difference between means by t-tests. Values of p < 0.05 were considered signi cant. To probe how NO regulates the development of lamentous fungi, we conducted the culture of onion pathogenic S. eturmiunum by supplementing SNP. Under laboratory growth conditions, the fungal colony was densely dotted with brown-colored conidia, and was more densely dotted upon exposure to 0.2 mmol/L SNP. However, the brown-colored conidia were reduced and gradually disappeared upon exposure to SNP at 2, 4, and 8 mmol/L, respectively (Fig. 1A).

Results
Next, we chose 0.2 mmol/L and 2 mmol/L SNP as the external NO source to observe NO-induced changes of phenotype. To con rm the regulatory roles of NO in the changes of phenotype, we also supplemented NO speci c scavenger cPTIO (1 mmol/L). The addition of cPTIO resulted in the retarded mycelial growth and the presence of more albinism mycelia on the surface of colonies especially in control and the cultures supplemented with 0.2 mmol/L SNP (Fig. 1B). To test the possible mechanisms of NO-induced phenotype changes of S. eturmiunum, we further used sGC speci c inhibitor NS-2080 (18 µmol/L) to block the formation of cGMP. Intriguingly, addition of NS-2080 resulted in the presence of more albinism mycelia and retarded mycelial growth in control cultures and the cultures containing 0.2 mmol/L SNP (Fig. 1B).
Involvements of NO in the formation of conidia and pseudothecia Morphologically, the produced conidia intertwine tightly with mycelia, and can hardly be isolated from cultures for counting. To this end, we portrayed conidiation qualitatively by visually comparing the density of the conidia present in the same square of culture plates in different treatments. In the control cultures, the promoted conidiation was observed upon exposure to 0.2 mmol/L SNP, and was largely reduced upon exposure to 2 mmol/L. The presence of cPTIO compromised conidiation in the SNPsupplemented cultures and totally abolished in control cultures. Intriguingly, application of NS-2080 resulted in the impairment of conidiation even in the presence of SNP ( Fig. 2A). SNP supplement also increased the formation of pseudothecia especially in the cultures exposed to 2 mmol/L SNP. Similarly, application of cPTIO and NS-2080 inhibited the formation of pseudothecia (Fig. 2B). To further identify the effects of NO on the formation of pseudothecia, we also prepared the cultures exposed to 4 mmol/L and 8 mmol/L SNP to observe the correlation of NO levels with the number of pseudothecia. As shown in Fig. 3A, the maximum number of pseudothecia was observed upon exposure to 2 mmol/L SNP and largely reduced in the cultures exposed to 4 and 8 mmol/L (Fig. 3A). Similar to conidiation, application of cPTIO and NS-2080 all reduced the number of pseudothecia especially in control and the cultures exposed to 0.2 mmol/L SNP (Fig. 3B).

External NO application changes the expression of genes involved in conidiation and the formation of pseudothecia
In Aspergillus molds, asexual development is orchestrated by BrlA, AbaA, and WetA transcriptional cascade (Lind et al. 2018). To testify the relevance between conidiation and expression of the three transcription factors in S. eturmiunum upon external NO application, we conducted the RT-PCR assay of the genes encoding BrlA (GenBank accession number: MT925646), AbaA (GenBank accession number: MT925645), and WetA (GenBank accession number: MT925644). SNP application at 0.2 mmol/L triggered the maximum increase in transcription levels of brlA, abaA, and wetA. Interestingly, application of cPTIO and NS-2080 all reduced expression levels down to 0.62 folds for brlA (Fig. 4A), 0.64 folds for abaA (Fig. 4B), and 0.59 folds for wetA (Fig. 4C), respectively. Similar to conidiation, exposure to 2 mmol/L SNP also caused the maximum increase in transcription levels of mat1 (up to 4.8 folds) and mat2 (up to 3.8 folds), the two genes involved in sexual reproduction, and reduced the expression levels of mat1 and mat2 upon application of cPTIO and NS-2080, respectively (Fig. 4D, F).

NO-stimulated biosynthesis of melanins correlates with increased conidiation and formation of pseudothecia
Biosynthesis of melanins in fungi plays a crucial role in defending fungal cells against environmental stresses. Accumulation of melanin in fungal propagules contributes to virulence and capacity to survive in harsh surroundings (Valiante et al. 2016). Interestingly, exposure to 2 mmol/L SNP stimulated production of melanins. Application of cPTIO and NS2080 compromised melanin biosynthesis especially in control and the cultures exposed to 0.2 mmol/L SNP (Fig. 5). To determine the possible types of melanins produced in S. eturmiunum, we further supplemented arbutin and tricyclazole, the two speci c inhibitors for DOPA and DHN biosynthetic pathways, respectively. Upon addition of arbutin or tricyclazole, the dark-brown colonies were bleached to albinism mycelia (Fig. 6A). In addition, supplement of the two inhibitors for melanin biosynthesis also impaired conidiation (Fig. 6B) and the formation of pseudothecia ( Fig. 6C, D).

NO production correlates with the biosynthesis of melanin in S. eturmiunum
NO is involved in many physiological processes of lamentous fungi and the production of NO has been demonstrated in many fungal species although the search for the genes coding for NOS-like proteins (NOSL) in fungal genomes remains unfruitful ). To test the capacity to produce NO by S. eturmiunum, we used the term "NO-producing capacity" to stand for NOS-like activity. In addition, we also assayed NO levels under the supplement of SNP, arbutin, and tricyclazole, respectively. Similar to other NO-producing lamentous fungi, NO-producing capacity was also observed in S. eturmiunum, and was reduced following supplement of SNP. Reduction in NO-producing capacity was also seen in the cultures supplemented with arbutin or tricyclazole. Intriguingly, simultaneous supplement of SNP and arbutin, or SNP and tricyclazole further reduced NO producing capacity (Fig. 7A). Accordingly, NO levels were also reduced evidently in the cultures supplemented with arbutin or tricyclazole (Fig. 7B). Notably, following the reduction in NO levels, melanin accumulation was decreased remarkably even in the presence of SNP (Fig. 7C). In order to further correlate NO production and melanin biosynthesis, we analyzed NO-producing capacity in 5-AC-treated S. eturmiunum. Obviously, 5-AC treatment resulted in the impairment in NO production, the activity of tyrosinase, as well as melanin biosynthesis, which coincides with the cultures supplemented with arbutin and tricyclazole (Fig. 8A, B). . Intriguingly, SNP treatment resulted in 9.4 folds increased transcription for pks1, 5.4 folds increased transcription for pks2, and 7.4 folds increased transcription for tyr. In contrast, 5-AC treatment down regulated l to 0.19 folds in transcription for pks1, 0.065 folds for pks2, and 0.094 folds for tyr (Fig. 8C). To further identify the function of pks1 and pks2, we also constructed the heterologous transformants of pks1 and pks2 using wA locus in Aspergillus nidulans LO8030. Heterologous expression of pks1 and pks2 in wA locus resulted in the presence of brown pigment in the conidia of either pks1 mutant or pks2 mutant (Fig. 9A). Moreover, the two transformants showed similar germination rate with conidia of A. nidulans after UV irradiation (Fig. 9B). Collectively, melanin biosynthesis is also dependent on cellular levels of NO in S. eturmiunum.

Discussion
The formation of conidia and pseudothecia of the onion pathogenic S. eturmiunum is the critical stage for its transmission. However, how the development of the two propagules is regulated remains to be fully understood. In the study, we showed that NO is necessary for conidiation and the formation of pseudothecia in S. eturmiunum. Application of NO scavenger cPTIO abolishes the formation of conidia and pseudothecia, as well as melanin production. In control cultures supplement of SNP results in an increased formation of conidia at 0.2 mmol/L, and pseudothecia at 2 mmol/L. SNP supplement also triggered increased biosynthesis of melanin, which can be inhibited upon addition of either arbutin or tricyclazole, the speci c inhibitors for DOPA and DHN melanin synthetic pathway, respectively. Moreover, the enhanced biosynthesis of melanin coincides with the increased formation of the two propagules that are impaired following the inhibition of melanin biosynthesis (Fig. 10).
The small free radical NO is a short-lived but highly reactive diatomic gas (Brüne 2010). Because it is highly diffusible within the cell and through cell membranes (Lancaster 1997), NO functions as a transient, local, intracellular or intercellular signaling molecule in diverse biological systems (Culotta & Koshland 1992). One of the important mechanisms that NO regulates physiological processes of living system is the binding of NO with transition metals of metalloproteins such as sGC, a hemoprotein that has evolved to bind selectively with NO (Boon & Marletta 2005). The activation of sGC by NO results in the production of the secondary messenger cyclic GMP (cGMP) (Friebe & Koesling 2003) that binds to protein kinase G (PKG), and forms the central downstream mediator of NO-cGMP signaling pathway, and mediates pathway-speci c cellular responses via the phosphorylation of phosphorylation-dependent transcriptional factors, such as the cAMP-response-element-binding protein (Contestabile 2008), and activates its downstream targets (Tomankova et al. 2017).
In lamentous fungi, endogenous production of NO correlates with mycelial growth and conidia formation (Marcos et al. 2020). In A. nidulans, increased production of NO was detected in the transition from vegetative growth to conidiation (Marcos et al. 2016). Similar to A. nidulans, our results showed that the presence of NO-producing capacity followed by intracellular production of NO correlates with the regular conidiation, which is compromised following the addition of NO scavenger cPTIO. This indicates that maintaining a certain level of cellular NO underpins the vegetative growth and asexual development in S. eturmiunum. Interestingly, addition of NO-releasing compound SNP resulted in an evident reduction in NO-producing capacity (Fig. 7A), which suggests that NO-producing capacity can be self-regulated in response to alteration of the cellular NO levels. In addition, SNP supplement at concentrations lower than 0.2 mmol/L also promotes conidiation, which implicates that external application of NO at lower concentrations favors the transcription of brlA, abaA, and wetA, the three transcriptional factors involved in conidiation (Chen et al. 2020).
Cellular NO levels also affect sexual development in lamentous fungi (reviewed by Zhao et al. 2020). In Aspergillus nidulans, the increase in cellular NO levels by disrupting the genes encoding avohemoglobin or supplementing NO-releasing compound promotes the formation of cleistothecia (Baidya et a., 2011). Similar to A. nidulans, supplement of SNP at 2 mmol/L increased transcription of mat1 and mat2 followed by increased formation of pseudothecia, which indicates that the higher NO levels also tend to induce sexual development in S. eturmiunum.
Melanins production in fungi is believed to protect hyphae and propagules from environmental stresses  (Engh et al. 2007). In Pestalotiopsis microspore, the production of polyketidederived DNH melanin is required for the formation of integrated conidia and viability in addition to morphogenesis, germination and viability (Yu et al. 2015). Moreover, production of DNH melanin is also linked to the development of sexual fruiting body, and is controlled by speci c regulatory genes involved in sexual differentiation in Sordaria macrospora (Engh et al. 2007). In our study, external addition of NO also promotes the transcription of the two genes encoding two polyketide synthases, and the gene coding for tyrosinase followed by increased melanin accumulation and formation of conidia and pseudothecia.
Notably, inhibiting biosynthesis of DOPA and DNH melanin all lead to the impairment in the formation of conidia and pseudothecia. This indicates that biosynthesis of both DOPA and DNH melanin is required for asexual and sexual development in S. eturmiunum.
The melanins present in fungal cells are involved in their protection from UV radiation desiccation, salinity and oxidation (Pacelli et al. 2020). Melanins in phytopathogenic or human pathogenic fungi are also involved in the protection against ROS attack from host defense (Papon et al. 2020). In lamentous fungi, most ascomycetes produce DHN-melanin (Gonçalves et al. 2012). While in the ubiquitous humanpathogenic fungus Aspergillus fumigatus, the pathogen that causes fatal lung infection in immunocompromised individuals, produces both DOPA and DHN melanins (Langfelder et al. 2003). The presence of DHN melanin in conidia protects from phagocytic uptake and ROS-induced intracellular killing by frugivorous amoeba Protostelium aurantium and disrupts its autonomous defense (Ferling et al. 2020). In Sporothrix schenckii, production of DOPA melanin in the presence of tyrosine in fungal cell confers more resistance to nitrogen-derived oxidants and UV irradiation (Almeida-Paes et al. 2012). In our study, heterologous expression of pks1 and pks2 all resulted in the production of pigmented conidia with resistance to UV irradiation. In this context, the production of DOPA and DHN melanins found in phytopathogenic S. eturmiunum and their tight connections with the formation of conidia and pseudothecia implicate that this fungus possesses more resistance to the attacks from environmental stressors than those producing DNH melanins alone.
The primary sensor of NO soluble guanylate cyclase (sGC) orchestrates NO-cGMP-PKG signaling pathway, and has been implicated in many essential physiological processes and disease conditions in mammals (Kang et al. 2019). Several studies have reported that sporulation in lamentous fungi is promoted by application of external NO but inhibited by sGC inhibitor L-NAME or ODQ. However, sporulation can be restored by exogenous cGMP (Zhao et al. 2020). In our study, NO promoted formation of conidia and pseudothecia, and melanin production can also be compromised by sGC speci c inhibitor NS-2080 even in the presence of SNP. This implicates the existence of NO-cGMP-PKG signaling pathway in S. eturmiunum that mediates the increased transcription of the genes encoding the downstream regulators for conidiation, formation of pseudothecia and melanin biosynthesis.
It should be noted that, in our study, in contrast to the increased formation of conidia and pseudothecia by lower concentrations of SNP (≤ 2 mmol/L), external supplement of SNP at higher concentrations (≥

Conclusion
Our results con rmed that NO is necessary for conidiation and the formation of pseudothecia in S. eturmiunum. Conidiation is promoted upon exposure to 0.2 mmol/L SNP, while pseudothecia formation is enhanced upon exposure to 2 mmol/L SNP. Application of NO scavenger cPTIO and sGC speci c inhibitor NS2080 abolishes their formation of conidia and pseudothecia, as well as melanin production. In addition, melanin accumulation in the fungus is achieved either by DOPA and DHN melanin synthetic pathway, which correlates with its asexual and sexual development, and confers the capacity for S. eturmiunum to transmit and infect effectively even in harsh environment.      Values are means ± SD (n=3), error bars represent SD. * P<0.05, ** P<0.01, *** P<0.001 by t test.