Abstract
Fusarium culmorum produces polyketide-structured aurofusarin and its precursor metabolites. Aurofusarin biosynthetic pathway is catalysed by the products of eleven genes located in gene cluster. In this study, the effects of the expression levels of Pks12, Gip6, and Gip7, responsible genes for the intracellular steps of the pathway, on pigmentation were investigated in an F. culmorum field isolate. Presence of three genes were determined via PCR and sequencing. Their expressions were investigated by qPCR at 48th, 72nd, 120th and 168th hours. Aurofusarin and rubrofusarin production were verified by HPLC at the same time periods. Mycelial pigmentation, which was initially white, turned yellow, then carmine red during the seven-day culture. Pks12, Gip6, Gip7 genes with 1282, 449 and 1278 bps had sequence similarities (86,6%, 99,4% and 80,5% respectively) with the genes of reference (FcUK99). The ΣCp values of all genes ranged from 29th to 32nd cycles, whereas the Σ∆∆Ct values were calculated between 9,59 E-02 and 1,30 E-02. Relative quantification revealed these genes were controlled by down-regulation compared to the β-tubulin expression. Aurofusarin quantities ranged from 2,355 ppm to 27,350 ppm between the 72nd and 168th hours whereas the yield of rubrofusarin decreased from 0,098 ppm to 0,063 ppm. (4) Conclusion: This study becomes first report for both investigating the expression levels of the genes responsible for the catalysis of intracellular steps of aurofusarin biosynthesis in F. culmorum, and for examining the relationship between gene expression and mycelium pigmentation.
Keywords:
Fusarium culmorum 1; aurofusarin 2; mycelial pigmentation 3; qPCR 4; HPLC-DAD 5
HIGHLIGHTS
• Molecular analysis of aurofusarin biosynthesis in F. culmorum.
• Mycelial pigmentation depending on gene expression and aurofusarin accumulation.
• Pigmentation variations depending on growth phase.
INTRODUCTION
Polyketide-structured aurofusarin is one of the secondary metabolites produced by F. culmorum [11 Ashley JN, Hobbs BC, Raistrick H. Studies in the biochemistry of microorganisms LIII. The crystalline colouring matters of Fusarium culmorum (W.G. Smith) Sacc. and related forms. Biochem J. 1937;31:385-97.]. Aurofusarin and its precursors participate in the formation of mycelium pigmentation [22 Medentsev AG, Yu Arinbasarova A, Akimeto VK. Biosynthesis of Naphthoquinone Pigments by Fungi of the Genus Fusarium. Appl Biochem Microbiol. 2005;41:503-7.,33 Frandsen RJ, Nielsen NJ, Maolanon N, Sørensen JC, Olsson S, Nielsen J, Giese H. The biosynthetic pathway for aurofusarin in Fusarium graminearum reveals a close link between the naphthoquinones and naphthopyrones. Mol Microbiol. 2005;61:1069-80.]. Mycelium pigmentation may have wide range of color which differs from yellow to carmine red depending on nutrient medium [55 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. Functional Characterization of Genes Located at the Aurofusarin Biosynthesis Gene Cluster in Gibberella zeae. Plant Pathol. 2008;24:8-16.]. The eleven genes responsible for aurofusarin biosynthesis are located as a gene cluster in the genome, and biosynthesis is carried out with multiple enzymatic steps. Nine of the eleven genes encode well described proteins while two encode hypothetical proteins. Their functions were identified through deletion mutant experiments [33 Frandsen RJ, Nielsen NJ, Maolanon N, Sørensen JC, Olsson S, Nielsen J, Giese H. The biosynthetic pathway for aurofusarin in Fusarium graminearum reveals a close link between the naphthoquinones and naphthopyrones. Mol Microbiol. 2005;61:1069-80., 55 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. Functional Characterization of Genes Located at the Aurofusarin Biosynthesis Gene Cluster in Gibberella zeae. Plant Pathol. 2008;24:8-16.-66 Frandsen RJ, Schütt C, Lund BW, Staerk D, Nielsen J, Olsson S, et al. Two novel classes of enzymes are required for the Biosynthesis of Aurofusarin in Fusarium graminearum. J Biol Chem. 2011;286(12):10419-28.]. Pks12, Gip6 and Gip7 encode critical enzymes that catalyze the intracellular steps of aurofusarin biosynthesis. The type-I polyketide synthase, encoded by Pks12 gene, is responsible for the catalysis of the condensation reaction between one acetyl-CoA and six manonyl-CoA units as the first step of the biosynthetic pathway. A yellow pigment, YWA1, is produced as the result of this reaction [66 Frandsen RJ, Schütt C, Lund BW, Staerk D, Nielsen J, Olsson S, et al. Two novel classes of enzymes are required for the Biosynthesis of Aurofusarin in Fusarium graminearum. J Biol Chem. 2011;286(12):10419-28.]. Gip6 encodes the dehydratase required for the dehydration of YWA1 to nor-rubrofusarin, the precursor metabolite of aurofusarin [66 Frandsen RJ, Schütt C, Lund BW, Staerk D, Nielsen J, Olsson S, et al. Two novel classes of enzymes are required for the Biosynthesis of Aurofusarin in Fusarium graminearum. J Biol Chem. 2011;286(12):10419-28.]. The conversion of nor-rubrofusarin to rubrofusarin - another yellow colored polyketide metabolite - is carried out by the activity of O-methyltransferase, encoded by Gip7 gene [33 Frandsen RJ, Nielsen NJ, Maolanon N, Sørensen JC, Olsson S, Nielsen J, Giese H. The biosynthetic pathway for aurofusarin in Fusarium graminearum reveals a close link between the naphthoquinones and naphthopyrones. Mol Microbiol. 2005;61:1069-80., 55 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. Functional Characterization of Genes Located at the Aurofusarin Biosynthesis Gene Cluster in Gibberella zeae. Plant Pathol. 2008;24:8-16.]. Pumping of rubrofusarin across the cell membrane, dimerization of two rubrofusarin metabolites, and modification of the aurofusarin are carried out through the enzymes encoded by the remaining genes in the gene cluster. Knowledge about the relationship between expression levels of the mentioned genes and mycelial pigmentation remains limited. There are not any studies in literature for revealing the expression levels of aurofusarin genes contributing to the formation of mycelial pigmentation with in relation to the growth phases of F. culmorum before.
The present study investigates the effects of the alterations in the expression levels of Pks12, Gip6 and Gip7 genes - responsible for the intracellular steps of the production of aurofusarin and its precursors - on mycelial pigmentation. Each of these genes were amplified from an F. culmorum genome, then verified via sequencing. Their expression levels were determined by qPCR at the 48th, 72nd, 120th and 168th hours of the cultures. In vitro aurofusarin and rubrofusarin amounts were also detected with high performance liquid chromatography with diode-array detection (HPLC-DAD) at the same time marks.
MATERIAL AND METHODS
Pathogen cultivation and pigmentation monitoring
Gene expression and HPLC analyses were carried out from F. culmorum field isolate purified with single spore analysis. The isolate was reactivated from glycerol stock on synthetic nutrient agar (SNA) and then was transferred to potato dextrose agar (PDA). Fungal growth was carried out in controlled growth chamber at 25 ºC and 50% humidity for seven days. Radial growth rate was measured and pigmentation alterations were monitored.
Isolation of genomic DNA
Genomic DNA (gDNA) was isolated according to protocol of Aamir and coauthors (2015) with minor modifications [77 Aamir S. A rapid and efficient method of fungal genomic DNA extraction suitable for PCR based molecular methods. Plant Pathol Quar J. 2015;5(2):74-81.]. Seven-day-old fresh mycelia were frozen with liquid nitrogen and homogenized in porcelain mortar. The homogenate was suspended in 500 µl lysis buffer (100 mM Tris HCl, 50 mM EDTA, 3% SDS, pH 8,0) and transferred into microtubes. 500 µl of LiCl solution (8 M) was added into the solution and the tube was centrifuged at 10,000 xg for 1 min at room temperature. The aqueous phase was transferred into a new tube and an equal volume of chloroform:isoamyl alcohol (24:1) was added. Centrifugation was carried out at 10,000 xg for 10 min at room temperature. The supernatant was transferred into a new tube and ethanol precipitation was performed by adding a 2 × volume of absolute ethanol and a 1:10 volume of NaOAc (3 M). After incubation at -80 ºC for 30 min, gDNAs were precipitated by centrifugation at 10,000 xg for 10 min at room temperature. Quantitative and qualitative analyses of gDNAs were carried out with NanoDrop 2000 (Thermo, USA) and then the integrity of gDNAs were controlled with agarose gel electrophoresis.
PCR amplification, sequencing and alignment analysis of aurofusarin genes
The Pks12, Gip6 and Gip7 were amplified via PCR by using specific oligonucleotides. The partial sequences of the genes (FG02324, FG02325 and FG02326) belonging to F. graminearum PH-1 were obtained from the National Center for Biotechnology Information (NCBI). Oligonucleotide primers were designed with the Primer3 program. Secondary structure and primer-dimer formations of the oligonucleotides were controlled with the oligoanalyzer tool of integrated DNA technologies (IDT) (Table 1). PCR components were mixed in a reaction volume of 25 µL including 1 × PCR buffer (Promega, USA), 2,5 mM MgCl2, 0,08 mM dNTPs, 10 mM of each primer, 50 ng of gDNAs and 0,02 U/µL of Taq DNA polymerase (Thermo, USA). The pre-denaturation of dsDNAs was carried out at 94 ºC for 5 min. Amplification was performed in 35 cycles at 94 ºC for 1 min, at 54-55 ºC for 1 min and at 72 ºC for 2 min. The final extension step was applied at 72 ºC for 10 min. Amplification products were visualized with agarose gel electrophoresis and were bidirectionally sequenced by using the Sanger method (ABI PRISM 3100 Genetic Analyzer, USA). ABI chromatograms of gene sequences were separately exported in the FASTA format via Chromas 2.6.6, then aligned with the sequences of the FcUK99 reference genome through CLUSTALW 2.6.6.
Total RNA extraction and cDNA synthesis
Total RNAs were extracted from the 48th-, 72nd-, 120th- and 168th- hour cultures by using the Tripure RNA isolation reagent (Roche, Switzerland). 50 mg of mycelium was homogenized with liquid nitrogen in a porcelain mortar. The manufacturer’s recommendations were followed as the isolation protocol. Quality and quantity of total RNAs were controlled with NanoDrop 2000 (Thermo, USA) and agarose gel electrophoresis. cDNA synthesis was carried out from total RNAs (2 µg) in a volume of 25 µl comprising of; 1 × reaction buffer, 60 µM random hexamer, 60 µM oligo-dT primer, 5 µM DTT, 1 U of protector RNase inhibitor, 1 mM dNTPs and 1 U reverse transcriptase (Roche, Switzerland). Synthesis reaction was performed in a thermal cycler (Biorad, France) in the following incubation steps; at 65 °C for 10 min, 55 °C for 30 min and 85 °C for 5 min.
qPCR analysis of Pks12, Gip6 and Gip7
TaqMan hydrolyse probes were used in the expression analysis of the genes. Oligonucleotide primers and probes were designed for each of the genes using the IDT PrimerQuest Tool. Secondary structure and primer-dimer formations were controlled with the oligoanalyzer tool of IDT (Table 2). qPCRs were set at 20 µl final volume comprising of probe master mix, 5 pmol of each primer and cDNA derived from 2 µg of total RNA. qPCR assays were maintained using the LightCycler 480 II system (Roche, Switzerland). Each experiment was repeated at least two times. Mean crossing point (ΣCp) values were recorded. Expression levels of the genes were normalized by comparing the ΣCp values of the housekeeping gene (β-tubulin) and ∆Cp values were calculated in accordance with the protocol proposed by Livak and Schmittgen [88 Livak KJ, Schmittgen TD. Analysis of relative gene expression data using real-time quantitative PCR and the 2(-Delta Delta C(T)) Method. Methods. 2001;25(4):402-8.]. Variance analysis was conducted on one-way ANOVA with Tukey’s post-test via Graphpad Prism 5.0 software.
Aurofusarin analysis by HPLC-DAD
The HPLC-DAD quantitative analysis was performed on a Shimadzu HPLC chromatographic system (Shimadzu Corporation, Kyoto, Japan), equipped with LC-20AD pumps, a DGU-20A model degasser unit, a SIL-20 HT autosampler, a CTO-10AS column oven and an SPD-M20A diode array detector. Mediterranean Sea 18 column, 150 mm length, 4,6 mm i.d. and 5 μm particle size were used. The mobile phase was a gradient prepared from deionized water (component A) and methanol containing 0,2% o-phosphoric acid (component B). All mobile phase solutions were filtered and degassed before use. The elution program was designed as follows: 0-14 min, 50% (B) to 100% (B); 14-18 min, 100% (B) to 50% (B), the total acquisition time was 20 min. The mobile phase flow rate was 1,0 mL/min, the column temperature was set at 30°C and the sample injection volume was 20 µl. Ultraviolet absorption was fixed at 250 nm. The standard stock solution of aurofusarin (100 mg/L), rubrofusarin (100 mg/L) and quercetin (I.S.) were prepared in acetic acid and stored at 4°C. HPLC-DAD analysis was carried out from the 48th-, 72nd-, 120th- and 168th-hour cultures depending on pigmentation profile.
RESULTS
Monitoring of pigmentation and observation of radial growth rate
Mycelium pigmentation was observed as white colour in the first 48 hours of cultivation. The radial growth rate of mycelium was measured 4,37 ± 0,35 cm in diameter at this stage corresponding to the lag phase and early log phase. At the center of the culture, the mycelia acquired yellowish pigmentation between the 48th and 72nd hours, included into the log phase, and the mean colony diameter was measured as 6,9 ± 0,42 cm in this period. Maximum radial growth rate (9 cm) was reached at 96th hour and the isolate entered stationary phase from the 120th hour onwards (Table 3). Mycelium pigmentation was observed as carmine red with yellow margins once the mycelium growth was limited. At the stationary phase (the 168th hour) all the pigmentation acquired as carmine red (Figure 1).
Amplification of Aurofusarin Genes and their Sequencing
Partial regions of Pks12 (1118 bp), Gip6 (593 bp) and Gip7 (1401 bp), belonging to the open reading frames (ORFs) of the genes, were amplified and sequenced by using specific oligonucleotide primers designed for this study (Figure 2). All chromatograms of nucleotide sequences belonging to the three genes had clear peaks without baseline noise. The 950 bp length fragments of Pks12 and Gip7, and 350 bp fragment of Gip6 were all aligned with the corresponding gene regions of the reference genome (FcUK99). The highest similarity value was found as 99,4% for the Gip6 gene, between the field isolate and the reference strain. Transversion and transmission type mutations were observed in Gip6. The nucleotide sequences of Pks12 and Gip7 genes were more polymorphic than that of the Gip6 gene of the field isolate. Similarity coefficients were calculated as 86,6% and 80,5% for Pks12 and Gip7, respectively. Sequences alignments revealed that transition and transversion type mutations are found in partial regions of both Pks12 and Gip7, while in-dels and SNPs occurred only in Gip7 gene (Figure 3).
Expressions of Pks12, Gip6 and Gip7 genes
ΣCp values revealed that the selected aurofusarin genes had already been transcribed when the mycelia had white pigmentation. Expression analysis also indicated that the expression levels of the three genes together with β-tubulin gradually decreased through lag phase to stationary phase. It was found that expression levels of Gip6 and Gip7 were higher than Pks12 at the lag phase and early log phase (Table 4). At the beginning of the stationary phase (the 120th hour) the expression level of Gip6 decreased more than Gip7 and Pks12. Pks12 and Gip7 decrease ratio were nearly the same as β-tubulin. ∆Cp values were calculated after normalization according to values of β-tubulin, the highest expression level was determined for Gip7 (1,68E-01) at the 168th- hour. The lowest expression level was also calculated for Gip7 (9,59E-02) at the 120th- hour. When the expressions of the aurofusarin biosynthetic genes were compared with the housekeeping gene, it was observed that fold change values of aurofusarin genes were nearly the same as that of the housekeeping gene (Table 4). Decrease in gene expression levels was observed at the 72nd hour. Expression levels of all genes increased at the 120th hour during stationary phase, and decreased again at the 168th hour (Figure 4A). Although relative quantification data indicated that the aurofusarin genes were down-regulated, all three genes were found to be transcribed even at the stationary phase (Figure 4B).
Aurofusarin Analysis by HPLC-DAD
Aurofusarin and rubrofusarin amounts were detected by HPLC-DAD at the 48th, 72nd, 120th and 168th hours corresponding to lag, log and stationary phases. The peaks were identified in comparison to the aurofusarin and rubrofusarin standards (Figure 5). HPLC-DAD analysis revealed that 4,717 ± 0,001 ppm aurofusarin and 13,443 ± 0,001 ppm rubrofusarin were found in the 48th-hour culture. The aurofusarin amount was determined as 2,355±0,001 ppm and the rubrofusarin amount was calculated as 0,098 ± 0,001 ppm at the 72nd- hour. Aurofusarin and rubrofusarin amounts were 4,742 ± 0,002 ppm and 0,068 ± 0,001 ppm respectively at the 120th- hour while they were measured as 27,350 ± 0,003 ppm and 0,063 ± 0,002 ppm respectively at the 168th- hour.
Mean linear growth rate (LGR) values (± SE) of the field isolate during 168 hours culturing SD: standard error
ΣCt (± SD) and ∆Cp values of Pks12, Gip6, Gip7 and β-tubulin as housekeeping gene SD: standard deviation; h: hour
Alignment data of partial fragment of Gip7 amplified from the field isolate with reference genome. * symbolizes homologue nucleotides - symbolizes in-dels
Relative expression patterns of the genes (A) and one-way ANOVA analysis of gene expressions of the Pks12, Gip6 and Gip7 genes, Bars represent standard errors; * p<0,5; **p<0,01; ***p<0,001 (B)
Chromatograms of standard mixture (A), 48th -hour culture (B), 72nd - hour culture (C), 120th -hour culture (D) and 168th -hour culture (E). Peaks were marked as 1. Quercetin I.S. (5 mg/L); 2.Aurofusarin (50 mg/L); 3.Rubrofusarin (5 mg/L)
DISCUSSION
Fusarium species synthesize aurofusarin and its precursor metabolites, which are responsible for mycelial pigmentation (yellow, tan, carmine red etc.) [44 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. GIP2, a Putative Transcription Factor That Regulates the Aurofusarin Biosynthetic Gene Cluster in Gibberella zeae. Environ Microbiol. 2006;72:1645-52.]. Their biosynthesis is carried out in intracellular and extracellular enzymatic steps. These enzymes are coded by eleven genes, which were analysed functionally via investigation of F. graminearum deletion mutants [33 Frandsen RJ, Nielsen NJ, Maolanon N, Sørensen JC, Olsson S, Nielsen J, Giese H. The biosynthetic pathway for aurofusarin in Fusarium graminearum reveals a close link between the naphthoquinones and naphthopyrones. Mol Microbiol. 2005;61:1069-80.
4 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. GIP2, a Putative Transcription Factor That Regulates the Aurofusarin Biosynthetic Gene Cluster in Gibberella zeae. Environ Microbiol. 2006;72:1645-52.
5 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. Functional Characterization of Genes Located at the Aurofusarin Biosynthesis Gene Cluster in Gibberella zeae. Plant Pathol. 2008;24:8-16.-66 Frandsen RJ, Schütt C, Lund BW, Staerk D, Nielsen J, Olsson S, et al. Two novel classes of enzymes are required for the Biosynthesis of Aurofusarin in Fusarium graminearum. J Biol Chem. 2011;286(12):10419-28.]. Pks12, Gip6 and Gip7, encode enzymes which participate intracellular steps of aurofusarin production, was revealed as responsible genes for mycelium pigmentation via presented alterations in previous quelling studies [33 Frandsen RJ, Nielsen NJ, Maolanon N, Sørensen JC, Olsson S, Nielsen J, Giese H. The biosynthetic pathway for aurofusarin in Fusarium graminearum reveals a close link between the naphthoquinones and naphthopyrones. Mol Microbiol. 2005;61:1069-80.
4 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. GIP2, a Putative Transcription Factor That Regulates the Aurofusarin Biosynthetic Gene Cluster in Gibberella zeae. Environ Microbiol. 2006;72:1645-52.-55 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. Functional Characterization of Genes Located at the Aurofusarin Biosynthesis Gene Cluster in Gibberella zeae. Plant Pathol. 2008;24:8-16., 99 Jin JM, Lee J, Lee YW. Characterization of carotenoid biosynthetic genes in the ascomycete Gibberella zeae. FEMS Microbiol Lett. 2010;302(2):197-202.]. Although it was initially reported that ∆Pks12 strains were incapable of synthesizing aurofusarin and exhibited milky white pigmentation [44 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. GIP2, a Putative Transcription Factor That Regulates the Aurofusarin Biosynthetic Gene Cluster in Gibberella zeae. Environ Microbiol. 2006;72:1645-52., 1010 Malz S, Grell MN, Thrane C, Maier FJ, Rosager P, Felk A, et al. Identification of a gene cluster responsible for the biosynthesis of aurofusarin in the Fusarium graminearum species complex. Fungal Genet Biol. 2005;42(5):420-33.], Jin and coauthors (2009) showed that ∆Pks12 were orange pigmented while the ∆gzcaRA/Pks12 and ∆gzcarB/Pks12 double mutants produced white pigments [99 Jin JM, Lee J, Lee YW. Characterization of carotenoid biosynthetic genes in the ascomycete Gibberella zeae. FEMS Microbiol Lett. 2010;302(2):197-202.]. Frandsen and coauthors (2006) detected yellow/green pigmented mycelia in ∆Gip7 due to the accumulation of nor-rubrofusarin, a precursor of aurofusarin [33 Frandsen RJ, Nielsen NJ, Maolanon N, Sørensen JC, Olsson S, Nielsen J, Giese H. The biosynthetic pathway for aurofusarin in Fusarium graminearum reveals a close link between the naphthoquinones and naphthopyrones. Mol Microbiol. 2005;61:1069-80.]. In another study, Frandsen and coauthors (2011) observed that the accumulation of another precursor, YWA1, resulted in brown/green pigmentation in ∆Gip6 mutant strains [66 Frandsen RJ, Schütt C, Lund BW, Staerk D, Nielsen J, Olsson S, et al. Two novel classes of enzymes are required for the Biosynthesis of Aurofusarin in Fusarium graminearum. J Biol Chem. 2011;286(12):10419-28.]. Interestingly, Cambaza and coauthors (2018) found that the mycelium of the same wild type isolate can exhibit different pigmentation profiles in the same culture conditions, changing from milky white to yellow to carmine red depending on growth phases during the cultivation [1111 Cambaza E, Koseki S, Kawamura S. The Use of Colors as an Alternative to Size in Fusarium graminearum Growth Studies. Foods. 2018;7(7):100-10.]. Despite all these findings, our understanding of Fusarium pigmentation mechanisms remains limited. Up until this study, the relationship between mycelium pigmentation and expression profiles of aurofusarin biosynthetic genes had not been clearly established. In this current study, in order to understand the role of Pks12, Gip6 and Gip7 on the alteration of pigmentation patterns in F. graminearum and for the first time in F. culmorum reference strains, expression levels of these genes were investigated at different growth phases. Despite F. culmorum genome not having been annotated yet, based on the alignment analysis conducted with the F. graminearum PH-1 genome, it is proposed that the aurofusarin gene cluster might also be responsible for pigmentation in F. culmorum. Oligonucleotide primers were designed according to the PH-1 aurofusarin gene cluster. These primers effectively amplified partial regions of the Pks12, Gip6, Gip7 (1458, 593, 1401 bps long, respectively). Through the sequencing and alignment analysis of all these amplicons, the presence of SNPs and in-del type mutations in F. culmorum was revealed (Figure 3). In spite of such variations, high sequence similarities (Table 4) were determined between F. culmorum and F. graminearum, suggesting that the Pks12, Gip6, Gip7 might be responsible for catalysing the intracellular reactions during aurofusarin biosynthesis in F. culmorum as well. Lind and coauthors (2017) reported that the synthesis of secondary metabolites in filamentous fungi may be affected by variations like SNPs [1212 Lind AL, Wisecaver JH, Lameiras C, Wiemann, P, Palmer, JM, Keller NP, et al. Drivers of genetic diversity in secondary metabolic gene clusters within a fungal species. PLoS Biol. 2017;15(11):e2003583.]. However, this current study shows that because SNPs and in-del type mutations in Pks12, Gip6 and Gip7 do not cause frameshift or alter ORFs, such variations do not hinder the production of aurofusarin.
Through qPCR and HPLC analyses, the production of aurofusarin and rubrofusarin was verified at the 48th, 72nd, 120th and 168th hours. In milky white pigmented mycelium, gene expression analyses showed all genes to have been transcribed by the 48th hour mark, and the highest rubrofusarin amount was calculated at that time point as 13,443 ± 0,001 ppm while aurofusarin was calculated as 4,717 ± 0,001 ppm. At log phase, during which growth rates reached their highest at around the 72nd hours, the mycelium pigmentation turned yellow as rubrofusarin amounts reached 0,098 ± 0,001 ppm, and aurofusarin amounts 2,355 ± 0,001 ppm. By the 120th hour, the beginning of the stationary phase during which the mycelium pigmentation was observed to be carmine red, aurofusarin amounts had already increased to 4,742 ± 0,002 ppm and continued to gradually increase up to 27,350 ± 0,003 ppm.
Vujakovic and coauthors (2017) determined that in vitro cultures of different Fusarium species able to be carmine red pigmented as a result of Pks12 expression, and a relationship between gene expression patterns and aurofusarin biosynthesis was suggested [1313 Vujanovic V, Daida MA, Prasad D. qPCR assessment of aurofusarin gene expression in mycotoxigenic Fusarium species challenged with mycoparasitic and chemical control agents. Biological Control. 2017;109:51-7.]. The present study revealed that in addition to Pks12 gene expression, the Gip6 and Gip7 expression patterns effectively contributed to aurofusarin biosynthesis, and that the accumulation of aurofusarin was responsible for the carmine red pigmentation. The relatively decreased expression of the Gip6 compared to the Pks12 and Gip7 at stationary phase explained why the concentration of nor-rubrofusarin in the cell was lower than that of rubrofusarin. It has been generally accepted that secondary metabolites are synthesized more at the stationary phase than at the log phase [1414 Vrabl P, Schinagl CW, Artmann DJ, Heiss B, Burgstaller W. Fungal Growth in Batch Culture - What We Could Benefit If We Start Looking Closer. Front Microbiol. 2017;16(10):2391-402.]. However, the qPCR results of this study showed the aurofusarin biosynthetic genes to have reached the highest expression levels in the log phase. Therefore, it was concluded that aurofusarin and rubrofusarin are also synthesized during the growth phase of F. culmorum, confirmed by HPLC data. As a precursor metabolite, rubrofusarin was detected more than aurofusarin in log phase. Throughout the stationary phase, more aurofusarin can be detected as rubrofusarin metabolites are dimerised.
In stationary phase, radial growth rate of the carmine red culture reached maximum value (9 cm). Cambaza and coauthors (2018) had previously reported that when the in vitro culture of F. graminearum reached its maximum diameter, mycelium turned carmine red and became darker [1111 Cambaza E, Koseki S, Kawamura S. The Use of Colors as an Alternative to Size in Fusarium graminearum Growth Studies. Foods. 2018;7(7):100-10.]. It was showed with the current study that F. culmorum reached maximum growth rate faster than and went down to stationary phase earlier than F. graminearum. Growth dynamics in fungal cultures depend on many environmental factors such as time of nutrient exhaustion, reutilization of excreted metabolites and previous cultural conditions of inoculum [1414 Vrabl P, Schinagl CW, Artmann DJ, Heiss B, Burgstaller W. Fungal Growth in Batch Culture - What We Could Benefit If We Start Looking Closer. Front Microbiol. 2017;16(10):2391-402.]. Therefore, different Fusarium species can exhibit different in vitro growth rates, and in vitro growth might correlate with in vivo pathogenicity of Fusarium isolates [1515 Brennan J, Fagan B, van Maanen A. Studies on in vitro Growth and Pathogenicity of European Fusarium Fungi. Eur J Plant Pathol. 2003;109:577-87.]. The isolate used in this current study was purified from corn, and may have different virulence and aggressiveness compared to laboratory strains used in previous studies. This may lead to differences among the growth rates of the isolates.
Secondary metabolite biosynthesis and the gene expressions coding the enzymes responsible for the catalysis of biosynthetic steps can be affected by cellular and environmental factors, and can vary even at different growth phases in culture. Medentsev and coauthors (1993) associated the increasement of aurofusarin biosynthesis in the stationary phase of in vitro culture with excess oxidative stress and the inhibition of respiration caused by decreased nitrogen and phosphorus sources [22 Medentsev AG, Yu Arinbasarova A, Akimeto VK. Biosynthesis of Naphthoquinone Pigments by Fungi of the Genus Fusarium. Appl Biochem Microbiol. 2005;41:503-7.]. Gmoser and coauthors (2017) mention that pigment production in filamentous fungi increases in response to oxidative stress. Therefore, it should be considered that the increasement of Pks12, Gip6 and Gip7 expressions at the 120th hour and the increasement of aurofusarin levels towards the 168th hour might have been triggered by increasing oxidative stress due to the ageing of the culture [1616 Gmoser R, Ferreira JA, Lennartsson PR. Filamentous ascomycetes fungi as a source of natural pigments. Fungal Biol Biotechnol. 2017;4:4.].
Jung and coauthors (2006) noted an increase in the expression of Pks4 and Pks13 responsible for the synthesis of zearalenon (ZEA), a polyketide-structured mycotoxin. ZEA was synthesized in ∆Pks12 mutants, whereas no ZEA production occurred in the overexpression mutants of Pks12, which cause large quantities of aurofusarin synthesis. It was also reported that ZEA is synthesized at the log phase as aurofusarin is synthesized at the stationary phase antagonistically [1717 Jung SK, Kim JE, Yun SH, Theresa L. Possible negative effect of pigmentation on biosynthesis of polyketide mycotoxin zearalenone in Gibberella zeae. J Microbiol Biotechnol. 2006;16:1392-8.]. Jung and coauthors [1717 Jung SK, Kim JE, Yun SH, Theresa L. Possible negative effect of pigmentation on biosynthesis of polyketide mycotoxin zearalenone in Gibberella zeae. J Microbiol Biotechnol. 2006;16:1392-8.] (2006)’s data line up with this study’s findings that the expressions of Pks12, Gip6 and Gip7 decrease at the 72nd hour when rapid mycelium growth occurs, and that higher aurofusarin levels are detected at the 120th hour when the gene expression levels increase.
Because Pks12, Gip6 and Gip7 are regulated by the transcription factor encoded by Gip2 of the same gene cluster [55 Kim JE, Jin J, Kim H, Kim JC, Yun SH, Lee YW. Functional Characterization of Genes Located at the Aurofusarin Biosynthesis Gene Cluster in Gibberella zeae. Plant Pathol. 2008;24:8-16.], the expression levels of all three genes fall at the 72nd hour, are upregulated at the 120th hour, and fall back again at the 168th hour.
CONCLUSION
In conclusion, a positive correlation among gene expression levels, growth phases, and mycelium pigmentation profiles was thus established. The present study revealed for the first time that F. culmorum went into stationary phase earlier than F. graminearum upon reaching the maximum radial growth rate faster, and that Pks12, Gip6 and Gip7 are also responsible for the catalysis of intracellular reactions of the aurofusarin biosynthetic pathway in F. culmorum. Effects of the expressions of other genes found in this cluster on pigmentation should be investigated alongside other factors impacting pigmentation. Determination of aurofusarin and rubrofusarin concentration accumulated in mycelia during the growth phases provide useful knowledge for proper timing and environmental conditions of large-scale production of these pigment molecules.
Acknowledgments:
The authors are grateful to Prof. Dr. Berna Tunali from the Department of Plant Protection, Agricultural Faculty, Ondokuz Mayis University, Samsun/Turkey, who purified the isolate previously.
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Funding: This research was funded by THE SCIENTIFIC AND TECHNOLOGICAL RESEARCH COUNCIL OF TURKEY, grant number 216Z007.
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Publication Dates
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Publication in this collection
27 Jan 2023 -
Date of issue
2023
History
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Received
20 Dec 2021 -
Accepted
12 Oct 2022