Peptide Synthetase Gene in Trichoderma virens

doi:10.1128/AEM.67.11.5055-5062.2001

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Applied and Environmental Microbiology, November 2001, p. 5055-5062, Vol. 67, No. 11
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.11.5055-5062.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Peptide Synthetase Gene in Trichoderma virens

S. E. Wilhite,¹ R. D. Lumsden,² and D. C. Straney¹^,^*

Department of Cell Biology & Molecular Genetics, University of Maryland, College Park, Maryland 20742-5815,¹ and Biocontrol of Plant Disease Laboratory, USDA Agricultural Research Service, Beltsville, Maryland 20705²

Received 4 April 2001/Accepted 18 August 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Trichoderma virens (synonym, Gliocladium virens), a deuteromycete fungus, suppresses soilborne plant diseases caused by anumber of fungi and is used as a biocontrol agent. Several traitsthat may contribute to the antagonistic interactions of T. virenswith disease-causing fungi involve the production of peptide metabolites(e.g., the antibiotic gliotoxin and siderophores used for ironacquisition). We cloned a 5,056-bp partial cDNA encoding a putativepeptide synthetase (Psy1) from T. virens using conserved motifsfound within the adenylate domain of peptide synthetases. Sequencesimilarities with conserved motifs of the adenylation domain,acyl transfer, and two condensation domains support identificationof the Psy1 gene as a gene that encodes a peptide synthetase.Disruption of the native Psy1 gene through gene replacement wasused to identify the function of this gene. Psy1 disruptants producednormal amounts of gliotoxin but grew poorly under low-iron conditions,suggesting that Psy1 plays a role in siderophore production. Psy1disruptants cannot produce the major T. virens siderophore dimerumacid, a dipetide of acylated N-hydroxyornithine. Biocontrol activity against damping-off diseasescaused by Pythium ultimum and Rhizoctonia solani was not reducedby the Psy1 disruption, suggesting that iron competition throughdimerum acid production does not contribute significantly to diseasesuppression activity under the conditionsused.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Trichoderma virens (synonym, Gliocladium virens [30]) is an effective biological control agent for plant diseases causedby soilborne fungi (26). The disease-suppressive ability ofT. virens is presumably related to its antagonistic behavior towardsother fungi. Multiple traits may contribute to this antagonisticactivity, particularly since the modes of interaction appear todiffer for different target fungi (17). Production of gliotoxin,an epidithiodiketopiperazine antibiotic, is associated with T.virens suppression of damping-off caused by Pythium ultimum (24,25, 37). Production of additional antibiotics, competitionfor resources in the soil or rhizosphere, and hyperparasitismof target fungi are traits that may account for other antagonisticinteractions (7). Cloning of genes associated with antagonistictraits could permit manipulation of the genes in T. virens andcould increase the biocontrol activity of thisorganism.

Small peptides are associated with a number of the traits that might contribute to T. virens biocontrol activity. Gliotoxinis a modified cyclic phenylalanine-serine dipeptide (19). Fungalsiderophores involved in iron uptake, a potential means of competitionin the soil, are commonly short peptides containing nonproteinamino acids (22). T. virens produces three types of hydroxamatesiderophores: a monohydroxamate (cis- and trans-fusarinines),a dipeptide of trans-fusarinine (dimerum acid), and a trimer disdepsipeptide(copragen) (18). Peptide toxins and siderophores in bacteriaand fungi often are produced nonribosomally by large multifunctionalpeptide synthetases. The enzymes are organized into repetitivesynthase units, each of which has the functions required to completea different single amino acid elongation step in the synthesisof the peptide product (20). The number and linear order ofthe repetitive synthase units correspond to the amino acid sequenceof the peptide product. The functions of each synthase unit includeATP-dependent activation of the amino acid, transfer of the acyladenylates to specific thiols located on enzyme-bound cofactors(4'-phosphopantetheine), and condensation to form a peptide bond;separate domains within the synthase unit perform these functions(the acylation domain, the acyl carrier domain, and the condensationdomain, respectively) (20).

The conservation of consensus signature sequence motifs, along with their spatial separation (20, 32, 34), providesa tool for cloning peptide synthetases in other organisms. Inthis study our objectives were to clone a peptide synthetase fromT. virens and to use specific gene replacement to identify thefunction of the cloned gene and its role, if any, in biocontrolactivity.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Fungal isolates and inoculum. T. virens G20-4VIB is a single-spore isolate of strain G20 (= GL21) (24). Non-gliotoxin-producing UV-induced mutants wereproduced in a previous study (37). T. virens strains, P. ultimumPuZS1, and Rhizoctonia solani Rs-23A (24) were maintained onV8 juice agar. (200 ml of V8 juice per liter, 3 g of CaCO₃ perliter, 20 g of agar perliter).

Isolation of a peptide synthase gene fragment by PCR. A PCR was performed with a T. virens G20-4VIB genomic DNA template primed with two degenerate oligonucleotides correspondingto conserved amino acid residues of peptide synthetases (34).Primer A was based on the GKPKG sequence in core C (5'-GGNAAPCCNAAPGG,where N is A, G, C, or T, P is A or G, and Y is C or T). PrimerB was based on the YKTGD sequence in core F (5'-PTCNCCNGTYTTPTA).The PCR was carried out in a 50-µl (total volume) mixture containing100 ng of genomic DNA, 200 pmol of each primer, 1.5 mM MgCl₂,and 2.5 U Taq of DNA polymerase. The thermal program was 40 cyclesof 1 min at 94°C, 1.5 min at 37°C, and 2 min at 72°C. The finalcycle was followed by 7 min of incubation at 72°C. An approximately700-bp product was cloned into the pCRII vector (Invitrogen, Carlsbad,Calif.) by using T/A overhang ligation according to the manufacturer'sdirections, resulting inpPCR675.

cDNA library construction and screening. Total RNA was isolated from individual 100-ml cultures of G20-4VIB grown in malt extract medium (1 × 10⁵ conidia/ml of inoculum) at 160 rpm and 24°C in the dark and harvested24, 28, 33, 39, and 49 h after inoculation. RNA isolation wascarried out essentially as described by Chomczynski and Sacchi(6). Polyadenylated mRNA was isolated with oligo(dT)-cellulosespin columns (mRNA separator kit; Clontech, Palo Alto, Calif.)by following the manufacturer's instructions. A custom directional,deoxyribosylthymine-primed cDNA library was constructed by Clontechin the $lambda$ ZAPII cloning vector. The custom library consisted of2 × 10⁶ independent clones with an insert size range of 0.6 to 3.5 kb(average insert size, ~1.5kb).

A cDNA clone was isolated by hybridization of the 675-bp amplified fragment from pCR675 to 75,000 PFU of the unamplified cDNAlibrary in Escherichia coli XL1-Blue MRF'. The 675-bp clone wasused to generate a high-specific-activity riboprobe (~1.6 × 10⁹ cpm/µg). Positive plaques in replicate filters were subjectedto secondary screening to isolate a single hybridizing plaque.In vivo excision using ExAssist/SOLR (Stratagene, La Jolla, Calif.)produced the cDNA insert in a pBluescript vector,pPsy1.

Southern blotting. Fungal DNA was isolated (35) for Southern blot analysis (29) by capillary transfer to MagnaGraph nylon membranes (MSI,Westboro, Mass.) and UV cross-linking in a Strata-linker (Stratagene).Hybridizations were performed in a solution containing 6× SSPE(1× SSPE is 0.18 M NaCl, 10 mM NaH₂PO_4, and 1 mM EDTA [pH 7.7]),2× Denhardt's reagent, 0.5% sodium dodecyl sulfate (SDS), 100µg of single-stranded DNA per ml, and 50% formamide at 42°C. Membraneswere prehybridized for 3 h prior to addition of fresh hybridizationsolution containing (per milliliter) 1 × 10⁶ to 5 × 10⁶ cpm of radioactively labeled DNA probe prepared by using a randomoligonucleotide labeling kit (Pharmacia, Piscataway, N.J.) asrecommended in the manufacturer's protocol. Following overnighthybridization at 42°C, the membranes were washed at 65°C in 2×SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate) for 30min, in 2× SSC-1% SDS for 30 min, and in 0.1× SSC-0.1% SDS for10 to 30min.

T. virens transformation. Protoplasts were prepared as described by Thomas and Kenerley (33), except that conidia (1 × 10⁶ conidia/ml) were germinated in a malt extract broth for 12 hat 28°C. This procedure generally yielded 1 × 10⁸ to 2 × 10⁸ protoplasts, which was adequate for two to four individual transformationsat a level of 5 × 10⁷ protoplasts pertransformation.

The transforming construct for gene disruptions was prepared by inserting a selectable marker into pPsy1. A 3.3-kb NarI fragmentof pCPGHY1 (5), containing the E. coli hygromycin B phosphotransferasegene (hygB) flanked by the Cryphonectria parasitica glyceraldehyde-3-phosphatedehydrogenase gene (Gpd1) promoter and terminator, was insertedinto a ClaI site of Psy1 (between the C and D motifs in the adenylatedomain). The resulting construct was confirmed by restrictionanalysis of plasmid DNA and was designated pPS-HYG1. The DNA usedfor transformation was a linear fragment produced by PCR amplificationfrom pPS-HYG1 with primers located near the termini of the clonedPsy1 cDNA, which eliminated the bacterial vectorsequences.

Transformation of protoplasts was performed by using a modification of the method of Thomas and Kenerley (33), as follows.A total of 1 × 10⁷ to 5 × 10⁷ protoplasts in an MES [2-(N-morpholino)ethanesulfonic acid]-bufferedosmoticum (50 mM MES, 50 mM CaCl₂, 0.5 M mannitol) were mixedwith 1 µg of the linear transforming construct in a 0.6-ml preparationand incubated for 20 min on ice and then for 20 min at room temperature.An equal volume of 40% polyethylene glycol 8000 in MES osmoticumwas added, and aliquots of the suspension were transferred to20 petri plates, each containing 25 ml of molten regenerationmedium (1 g of yeast extract per liter, 1 g of casein hydrolysateper liter, 342 g of sucrose per liter, 16 g of agar per liter).After incubation at 28°C for 6 to 12 h, each of the plates wasoverlaid with 25 ml of molten water agar containing 600 µg (215U) of hygromycin B (Calbiochem, La Jolla, Calif.) per ml. HygromycinB-resistant colonies were recovered after 2 to 3 days of incubationat 28°C. Single-spore isolates were recovered from hygromycinB-resistant colonies. Transformant stability was determined byfour successive passages of conidia on nonselective potato dextroseagar, followed by plating of 100 conidia from each isolate ontopotato dextrose agar plates with and without 500 µg of hygromycinB perml.

Siderophore production and determination. Spores were inoculated into the following low-iron medium (2), which is similar to the Grimm-Allen medium used previouslyfor induction of siderophore production in T. virens (18). Autoclavedbase medium (1 g of K₂SO₄ per liter, 1 g of K₂HPO₄ per liter,3 g of ammonium acetate per liter, 1 g of citric acid per liter,2 mg of ZnSO₄ · 7H₂O per liter, 80 mg of MgSO₄ · 7H₂O per liter)was supplemented with (per liter) 20 g of sucrose, 1 ml of a traceelement solution (carbon-free trace elements [2] minus iron),and 1 ml of a stock vitamin solution (0.1 mg of biotin per ml,2 mg of myo-inositol per ml, 2 mg of thiamine HCl per ml, 1 mgof p-aminobenzoic acid per ml, 1 mg of pantothenic acid per ml,1 mg of nicotinamide per ml, 1 mg of pyridoxine HCl per ml), andthen the pH was adjusted to 6.8 with NH₄OH. High-iron medium wasprepared by supplementing this base medium with FeSO₄ · 7H₂O (55.6mg/liter).

Siderophore contents in culture filtrates were measured by measuring total hydroxamate contents (2). In this assay, 0.2ml of a culture filtrate was mixed with 1 ml of 5 mM Fe(ClO₄)₃,and the optical density at 500 nm was determined by using a blankprepared from sterile medium. Values are expressed below in millimolarequivalents of ethylenediamine-di(o-hydroxyphenylacetic acid)(Sigma Chemical Co., St. Louis, Mo.), a synthetic hydroxamatestandard, as measured with a standard curve. For partial purificationand thin-layer chromatography (TLC) analysis of dimerum acid (18)we utilized 18 ml of culture filtrate evaporated in vacuo. Theremaining gum was extracted in 6 ml of methanol overnight at roomtemperature and filtered through miracloth (Calbiochem) to removeundissolved material. Six hundred milligrams of XAD-2 resin (Supelco,Bellefonte, Pa.) was added to the sample, which shaken in an orbitalshaker for 24 h at room temperature (25 to 28°C). The solventwas collected by filtration through miracloth, and more XAD-2resin (600 mg) was added to the solvent. After a second filtration,the XAD-2 resin from the two extractions was combined in a 3-mlcolumn, washed with 12 ml of distilled water, and eluted with12 ml of methanol. Dimerum acid was released in the methanol extraction,while trans- and cis-fusarines were partially lost in the waterwashes (18). The methanol extract was dried, resuspended in20 ml of methanol, and subjected to TLC on silica plates (60A;Whatman) with a chloroform-methanol-water (35:12:2) solvent. Hydroxamateswere visualized by spraying the plates with 5 mM Fe(ClO₄)₃.

Biological control assays. The biological control assays used were assays that were modified from the assays described by Lumsden and Locke (24). Theantagonist inoculum used for biological control assays was preparedby transferring the conidia from one V8 juice agar slant (18-mmtest tube) into 60 g of autoclaved bran (ratio of bran to H₂O,1:1 [wt/vol]) and incubating the preparation in the light at roomtemperature for 3 days. An R. solani inoculum was prepared bymixing autoclaved RE/CM (20 g of RediEarth [W.R. Grace & Co, Columbia,Md.], 0.4 g of 80-mesh cornmeal, 60 ml of water) with a 3-day-oldagar plate culture and incubating the mixture at room temperaturefor 10 days. A P. ultimum inoculum was prepared by mixing autoclavedSCM (200 g of coarse sand, 6 g of coarse-ground cornmeal, 40 mlof water) with an agar plate culture and incubating the mixtureat room temperature for 2 weeks. For each treatment, soillessmix (360 g of RediEarth, 720 ml of water containing 1.5 g of 20-10-20N-P-K fertilizer) was amended with antagonist and pathogenic isolates(10 g of T. virens-colonized wheat bran and 1.8 g of R. solaniRediEarth-cornmeal inoculum or 8.0 g of P. ultimum sand-cornmealinoculum). All ingredients were mixed in large plastic bags andincubated for 10 to 13 days at 30°C. The bags were shaken at theend of the incubation period, and then the mixture in each bagwas subdivided and placed into three planting flats (12 by 16cm; 300 g each) to obtain a total of three replicates per treatment.Three rows (10 seeds/row) of eggplant seeds were planted in eachflat, and the seedlings were examined after 2 weeks of incubationat 26 to 30°C (R. solani) or after 3 weeks of incubation at 24°C(P. ultimum) for disease incidence. The healthy control containedno fungal inoculum, whereas the disease control was treated withthe pathogen and sterile bran. Disease incidence was scored bydetermining the percentage of seedlings standing compared to thenumber of seeds planted (percentage of plant stand). A statisticalanalysis was carried out as described by Lumsden and Locke (24).

The pH of RediEarth was modified to decrease iron availability by adding Ca(OH)₂ dispersed in water at the rates indicatedin Table 1 4 days before fungal isolates were added. No fertilizerwas added to the RediEarth to avoid introducing contaminatingiron present in the fertilizer.

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TABLE 1. Relative biocontrol activities of T. virens strains carrying the Psy1 disruption compared to the activity of parental isolate G20-M37

Nucleotide sequence accession number. The nucleotide sequence of Psy1 has been deposited in the GenBank database under accession number AF351825.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Cloning and sequence analysis of Psy1. We used degenerate oligonucleotides corresponding to portions of conserved cores C and F of peptide synthetases to prime aPCR performed with T. virens genomic DNA. A fragment that was675 bp long, which is consistent with the expected size, was clonedand sequenced. The predicted amino acid sequence encoded by thisfragment exhibited extended sequence similarity with the sequenceof the HC peptide synthetase from Cochliobolus carbonum (31).The 675-bp fragment was used to screen 75,000 independent clonesof a polydeoxythymidylic acid-primed cDNA library prepared fromT. virens poly(A)⁺ RNA. This screening yielded one cDNA clone (pPsy1) with a 5,056-bpinsert. The cDNA insert possessed an open reading frame from the5' terminus corresponding to a 1,609-amino-acid protein fragmentwith a molecular mass of 178 kDa. Sequence similarity was observedin core consensus regions (Fig. 1) found in the adenylate domainsof bacterial peptide synthetases, including the C motif believedto be characteristic of peptide synthetase adenylate domains (36).In addition, domains for cofactor binding (acyl carrier domain)and condensation which are unique to peptide synthetases (20)were identified (Fig. 1). The organization of the domains comprisingthe synthetase unit (condensation-adenylation-cofactor binding)is similar to the organization of gramicidin S synthetase andtyrocidine synthetase 2 from Bacillus brevis and surfactin synthetases1, 2, and 3 from Bacillus subtilis (20). A second region withsequence similarity to the acyl carrier domain was located towardsthe N terminus of the Psy1-encoded fragment, which suggests thatthere is a second (and incomplete) synthase unit encoded upstreamof the cloned gene fragment. Optimized protein alignments of thePsy1-encoded fragment with known peptide synthetase domains offungal origin, obtained by using CLUSTAL W (European BioinformaticsInstitute [http://www2.ebi.ac.uk/clustalw]), revealed similarityto the consensus core sequences defining these domains (Fig. 1).The deviations from the consensus core sequences derived frombacterial genes were similar to those observed for the sequencesderived from other fungal genes and usually involved hydrophobicamino acid substitutions. The level of amino acid sequence identitybetween the Psy1-encoded fragment and the consensus sequence derivedfrom bacterial genes was 62% for the adenylate domain, comparedto 63 to 88% for Nid1 and Hts1; the level of amino acid sequenceidentity was 71% for the acyl carrier domain, compared to 57 to86% for Nid1 and Hts1 units; and for the condensation domain thelevel of identity was 31% and the level of similarity was 60%,compared to 21 to 43% identity and 45 to 55% similarity amongNid1 and Hts1 units.

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FIG. 1. Restriction map and modular organization of Psy1 with regions of high sequence similarity to conserved adenylate domain motifs. (a) Restriction map of the 5,056-bp cloned cDNA of Psy1. Abbreviations: B, BamHI; C, ClaI; E, EcoRI; H, HindIII; S, SalI; N, NarI; Xb, XbaI; Xh, XhoI. (b) Regions of similarity to consensus sequence motifs of bacterial peptide synthetases (20). (c) Sequences in the motifs compared for the adenylate domains of Psy1 and other fungal peptide synthetases. Shading indicates sequence identity with the bacterial consensus sequence (consen.). Sequence comparisons were carried out with CLUSTALW (European Bioinformatics Institute [http://www2.ebi.ac.uk/clustalw]), and the entire adenylate domains and acyl carrier domains were used to preserve relative spacing between blocks. The genes used were the genes for ferrichrome siderophore synthetase (Sid2) from U. maydis (GenBank accession no. U62738), ACV synthetase (Nid1) from Aspergillus nidulans (GenBank accession no. X54853), HC toxin synthetase (Hts1) from C. carbonum (GenBank accession no. M98024), and enniatin synthetase (Esyn1) from Fusarium avenaceum (GenBank accession no. Z18755). Each adenylate domain/acyl carrier domain in a gene is numbered in the order of its appearance in the gene. However, Psy1 acyl carrier domain 2 (Psy1-2) is the acyl carrier domain located at the 5' end of the cDNA and potentially is part of another incomplete synthetase unit. The relative organization of motifs is conserved in the adenylate domain; however, the organization of the condensation, adenylate, and acyl carrier domains is not the same for all genes.

Disruption of the Psy1 gene. Wild-type biocontrol strain G20-4VIB was transformed with gene disruption construct pPS-HYG1, in which the selectable marker(hygB) was inserted into the middle of the cloned Psy1 gene (Fig.2). Following production of single-spored hygromycin B-resistantisolates, we noticed that 11 of 168 isolates recovered germinatedbetter (80 to 100% germination) on the hygromycin B-containingmedium than the majority of the transformants germinated (<0.1%germination). These 11 isolates, six additional transformants,and G20-4VIB (untransformed) were analyzed by Southern blotting(Fig. 2B) for the expected integration. The untransformed G20-4VIBstrain had only one copy of Psy1 and produced a single HindIIIfragment (3.5 kb) when it was hybridized to the probe locatedat the 3' end of the gene. The G20-4VIB transformants that wereunstable in the presence of hygromycin B, T1 to T5 and T9, producedboth the native 3.5-kb fragment from the native gene and one ormore bands representing ectopic integrations of the transformingconstruct. All 11 isolates that were stable in the presence ofhygromycin B, T31, T34, T38, T104, T108, T109, T123, T130, T132,T155, and T168, lacked the 3.5-kb fragment associated with thenative gene and instead contained a single 6.3-kb fragment thatwas consistent with the expected gene replacement event resultingin disruption of the Psy1 gene (Fig 2B).

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FIG. 2. Disruption of the Psy1 gene in G20-4VIB (wild type) and non-gliotoxin-producing mutant G20-M37. (A) Gene disruption construct (pPS-HYGI) obtained by insertion of HygB (hygromycin phosphotransferase) expressed from the C. parasitica Gpd1 promoter (Gpd1::hygB) into the ClaI restriction site of the Psy1 cDNA insert in pPsy1. The positions of nucleotides corresponding to adenylate domain motifs A to O are indicated. PCR amplification with primers located at the termini of the Psy1 insert was used to produce a linear DNA fragment used for transformation to eliminate vector sequences. Insertion of the hygB cassette into native Psy1 resulted in a 2.8-kb increase in the size of the HindIII restriction fragment. (B) Southern blot analysis of HindIII-digested chromosomal DNA of T. virens wild-type strain G20-4VIB (lane WT) and transformants for detection of gene disruption events. Lane M contained molecular weight markers. (C) Southern blot analysis of HindIII-digested chromosomal DNA of T. virens wild-type strain G20-4VIB (lanes WT), gliotoxin mutant G20-M37 (lane M37), and G20-M37 transformants for detection of gene disruption events. Blots were probed with a ³²P-labeled PCR fragment corresponding to the 3' end of Psy1. Lane M contained molecular weight markers.

Effect of the Psy1 disruption on gliotoxin production. The abilities of the Psy1-disrupted isolates to produce gliotoxin were determined by TLC analysis of filtrates from 2-day-oldmalt extract broth (Difco, Detroit, Mich.) cultures. The Psy1disruptants displayed no decrease in gliotoxin production comparedto the wild-type strain, as determined by visual comparison ofthe bands on the plates by UV shadowing (Fig. 3) or after stainingfor gliotoxin with silver nitrate (37) (data not shown). Thelack of a change in gliotoxin levels was confirmed by gas chromatography-massspectrometry analysis of culture filtrates for gliotoxin. Theheights and elution times of the gliotoxin peak were similar inthe Psy1 disruptant and wild-type strains (data not shown).

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FIG. 3. Gliotoxin production in Psy1 disruptants of G20-4VIB. Filtrates from malt broth cultures grown for 2 days were extracted with chloroform and subjected to TLC on a plate with a fluorescent background (37). Dark bands indicate UV-absorbing compounds. Lane Std contained a gliotoxin standard. Culture filtrates of wild-type strain G20-4VIB (lane WT) and Psy1disruptants (T strains) derived from this strain were also included. The arrows indicate the positions of gliotoxin (G) and viridin (V). Viridin is a sterol metabolite that is not related to gliotoxin. Band MeG is dimethyl gliotoxin, an inactivated derivative of gliotoxin formed in culture.

Effect of Psy1 disruption on iron-dependent growth. When we cultured the transformants on Weindling's modified medium (a defined T. virens culture medium [37]) lacking theusual 3 µM Fe-EDTA supplement, we observed that the colonies ofall 11 Psy1 disruptants were smaller than the colonies of wild-typeT. virens or five ectopic transformants (T1 to T5). In contrast,the colony sizes were similar to the colony sizes for these otherstrains when the organisms were grown on Weindling's modifiedmedium containing the iron supplement. High iron levels (e.g.,micromolar) in the growth medium normally repress siderophoreproduction due to sufficient nonspecific iron transport, whilelow iron concentrations normally induce siderophore production(22). We more fully assessed the effect of Psy1 disruption onsiderophore production by examining two representative disruptants,T31 and T155. Siderophore production was measured by determining(i) the ability to grow (as measured by mycelial dry weight) ina liquid medium that minimizes levels of trace iron compared tothe ability to grow in the same medium supplemented with ironand (ii) the amount of hydroxamate siderophore produced in thelow-iron medium. Both growth and hydroxamate levels were monitoredfor 8 days in culture, after the rapid growthphase.

Compared to the wild type, both Psy1 disruptants grew poorly under low-iron conditions (Fig. 4A) but normally under high-ironconditions. This iron-dependent growth defect was not observedin six T. virens transformants that carried only an ectopic copyof the disruption construct and contained an intact Psy1 gene(data not shown). A general hydroxamate siderophore assay wasperformed with partially purified culture medium collected duringgrowth. In low-iron medium, in which siderophore production isnormally induced, hydroxamate siderophore was detected in Psy1disruptant T31, but the levels were 30-fold lower than the wild-typelevels (Fig. 4B). Although part of the loss of siderophore activitycould be attributed to the decreased growth in the low-iron medium,the amount of siderophore was at least eightfold lower in thedisruptants than in the G20-4VIB recipient strain when the valueswere normalized to the dry weights of mycelia recovered from thesame cultures. The other Psy1 disruptant, T155, displayed no detectablesiderophore production (Fig. 4B). TLC after XAD-2 resin purificationwas used to detect the hydroxamate dimerum acid in culture filtrates.Although dimerum acid was clearly detected in wild-type culturesand was present on days 4 to 8, it was not found in the Psy1 disruptantcultures (Fig. 4C and data not shown) in any of the samples collectedthrough day 10. Copragen was not detected in this assay, as expectedfrom the relatively low levels previously reported (18). Fusarinineswere not detected, as expected from their tendency to wash fromthe XAD-2 resin used in the purification process (18). TLC analysisof the methanol extracts without XAD-2 resin purification (datanot shown) indicated that a ninhydrin-stained compound remainedat the origin, which was consistent with the presence of trans-or cis-fusarinine. Such staining was observed with G20-4VIB, T31,and T155.

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FIG. 4. Mycelial growth, siderophore production, and dimerum acid levels in G20-4VIB and Psy1 disruptants. Spores of G20-4VIB (wild type) (circles) or Psy1 disruptants T31 (triangles) and T155 (squares) were inoculated into a base medium used to limit trace iron (<0.1 µM Fe), and the resulting cultures were divided into equivalent 10-ml cultures. Supplemental iron was added to one-half of the flasks to create high-iron conditions (100 µM Fe) (open symbols), while the other cultures were not supplemented in order to create low-iron conditions (solid symbols). Triplicate cultures were harvested by filtration at different times after inoculation for the wild-type and T31 strains. Duplicate cultures were harvested for strain T155. The dry weight of the mycelium in each 10-ml culture (A) and the total hydroxamate siderophore yield for each culture filtrate (B) are shown. To determine the total amount of hydroxamate utilized, we performed an Fe(ClO₄)₃ assay with samples of culture filtrate that were not purified. The error bars indicate standard errors of the mean. (C) Dimerum acid levels in the culture filtrates analyzed by methanol extraction, purification on XAD-2 resin, and TLC. The only band was the Fe(ClO₄)₃-stained band on TLC chromatograms, and this band comigrated with a dimerum acid standard. Lane C contained a control extraction of uninoculated culture medium.

Effect of the Psy1 disruption on biocontrol activity. We also generated a set of Psy1 disruptants in a gliotoxin mutant (glx) background G20-M37, a UV-induced glx mutant of G20-4VIB(37), in order to focus the biocontrol assays on differencesin siderophore production. Eight of the 80 single-spore transformantspossessed the stable hygromycin B-resistant phenotype, and sevenof these had the Psy1 disruption (Fig. 2C).

Biocontrol activities of the disruptants were tested by performing standard assays for suppression of pythium and rhizoctoniadamping-off (Table 1). One experiment showed that two Psy1 disruptantsreduced R. solani damping-off to some extent, but for replicatesof R. solani or P. ultimum there was no consistent reduction inbiocontrol activity compared to controls. We also tested biocontrolactivity under conditions that decreased the availability of ironby increasing the pH of the soilless mix (Table 2). For one Psy1disruptant of G20-4VIB, T155, there was a small but significantreduction at the highest pH, but there was not a consistent trendtoward less biocontrol activity in all replicates.

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TABLE 2. Relative biocontrol activities of G20-4VIB and T. virens Psy1 disruptants against pythium and rhizoctonia damping-off with different pH values

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The T. virens Psy1 gene that we cloned appears to encode a segment of a peptide synthetase. This gene is not involved in biosynthesisof the dipeptide antibiotic gliotoxin but instead appears to beassociated with production of a major siderophore, dimerum acid.We used Psy1 disruptants to test the role of siderophores in fungalbiocontrol activity. The retention of full biocontrol activityby the disruptants indicates that dimerum acid siderophore productionand perhaps iron competition are not limiting factors in the suppressionof rhizoctonia and pythium damping-off by T. virens under theconditionstested.

The Psy1 gene probably encodes a peptide synthetase. There is extended sequence similarity to the conserved motif of the adenylatedomain of peptide synthetases, particularly peptide synthetasesfrom other filamentous fungi, which are different from relatedadenylate-forming enzymes (34). The Psy1-encoded sequence alsocontains regions similar to two acyl carrier domains and a condensationdomain flanking the adenylate domain. The positions of these domainsare conserved in peptide synthetases (20), and this suggeststhat one complete synthase unit and part of a second synthaseunit are located near the N terminus of the translated peptide.The Psy1-encoded sequence also contains a region that matchesthe thioesterase/transferase consensus region (GXSXG) often foundnear the C termini of other peptide synthetases, including thepeptide synthetases for ACV, gramicidin S, and surfactin (20).Although the open reading frame fragment encoding 1,609 aminoacids is only a partial coding region, as expected from the largersizes of other peptide synthetases, the cloned fragment is largeenough to permit manipulation of the gene through targeted genedisruption (15).

Assuming that there are no redundant genes or partial activity of the disrupted gene, the continued production of gliotoxinby the Psy1 disruptants indicated that PSY1 is not involved inbiosynthesis of gliotoxin. Peptide synthetases are also involvedin synthesis of siderophores for iron uptake. T. virens producessiderophores that are monomers and multimers of the monohydroxamatescis-fusarinine and trans-fusarinine (18), which are N-acylated derivatives of N-hydroxylated ornithine, a nonproteinaceous amino acid. The fusarininesand the dihydroxamate (dimerum acid) constitute the majority ofsiderophores in T. virens, and each accounts for 45% of the totalsiderophore yield (18). The trihydroxamates copragen and copragenB account for about 6% of the totalsiderophores.

The Psy1 disruptants display several traits that are consistent with a large reduction in siderophore production. First, theygrow poorly in low-iron medium, and the defect appears to be adefect in iron acquisition. Second, the amount of total hydroxamatesiderophores is markedly decreased in the Psy1 disruptants, anddimerum acid is not present in culture filtrates. We infer fromthese findings that PSY1 is involved specifically in dimerum acidsynthesis. Previous studies with mycelial extracts of Fusariumcubensis, another producer of dimerum acid, detected ATP-pyrophosphateexchange in the presence of trans-fusarinine. These results suggestthat a peptide synthetase utilizes trans-fusarinine as a substrate(1). The loss of dimerum acid and the apparent presence ofthe monohydroxamates in the Psy1 disruptants are consistent withPSY1 being a peptide synthetase, presumably forming the cyclicpeptide bond from two trans-fusarinine molecules. The role ofPSY1 in synthesis of copragen or copragen B, which adds a thirdtrans-fusarinine in an ester linkage to dimerum acid, remainsto be determined. Such linkages can be produced by peptide synthetases(e.g., the depsipeptide enniatin [12]), but a peptide synthetaseother than that encoded by Psy1 may be responsible for copragensynthesis.

If the role of PSY1 is to produce a fungal hydroxamate siderophore, then it is surprising that the sequence of the PSY1 adenylatedomain is more similar to the sequences of the adenylate domainsof the C. carbonum HC toxin synthetase (47 to 54% similarity)than to the sequences of the adenylate domains of the Ustilagomaydis ferrichrome synthetase (42 to 47% similarity), the onlyother cloned fungal peptide synthetase that produces a siderophore.The differences may be attributable to the large differences inthe structures of these siderophores. Ferrichromes have otheracyl modifications of ornithine and additional neutral amino acidsin head-to-tail linkages as hexapeptides (22).

Competition for nutrients is thought to be one mechanism for antagonistic interactions between biocontrol agents and plantpathogens, and it has been proposed that siderophore productionis an important mode of competition for iron in the soil (23).Studies of bacterial biocontrol agents in which non-siderophore-producingmutants have been used have provided conflicting results in testsof this hypothesis. Pseudomonas aeruginosa mutants that lack siderophoreshave reduced biocontrol activity against Fusarium oxysporum (11),while similar Pseudomonas fluorescens and Pseudomonas putida mutantshave full biocontrol activity against Pythium aphanadermatum,P. ultimum, and Gaeumannomyces graminis var. tritici (21, 27,28). Manipulation of multiple siderophores in P. aeruginosa(4) and Enterobacter cloacae (8) has provided similarlydisparate results, indicating that the roles of siderophores maydepend on the pathogen-bacterial biocontrol agent pair. In ourtest of a fungal biocontrol agent, T. virens, we did not observeany consistent loss of biocontrol activity against either P. ultimumor R. solani, even when the soil pH was increased to reduce ironavailability. The biocontrol assay used, which involved preincubatingT. virens with the pathogen for 10 days prior to introductionof the plant, should have increased competition for iron in thesoilless mix. Production of dimerum acid does not appear to bea significant factor in the ability of T. virens to suppress pythiumor rhizoctonia damping-off. We cannot, however, rule out the possibilitythat conditions in the biocontrol assay enhanced production ofthe monohydroxamate siderophores in the Psy1 disruptants, compensatingfor the loss of dimerum acid. Cloning and disruption of a geneor genes encoding ornithine hydroxylation and acylation enzymesin T. virens are needed to test the role of fusarinine in biocontrolactivity. The clustering of ornithine-N⁵-oxygenase activity and the peptide synthetase for ferrichromesynthesis in U. maydis (22) suggests that a similar gene maybe located near Psy1 in T. virens.

Psy1 should be a useful tool for molecular definition of the diverse siderophores produced by fungi, particularly the ascomycetes,in which no other genes have been cloned (22). A range of fungiproduce copragen and dimerum acid; these fungi include the humanpathogen Histoplasma capsulatum (3, 16) and the plant pathogensVerticillium dahliae (13) and G. graminis var. tritici (10).Homologs of Psy1 may be present in these fungi and have a rolein animal or human pathogenicity, while the same siderophoresproduced by Penicillium chrysogenum increase iron utilizationby plants (14) and may have a role in plant growth promotionby this strain of T. virens (9). An intact Psy1 clone may beuseful in engineering hydroxamate siderophore production in plantsor in providing plant growth enhancement by T. virens beyond suppressionof disease-causingfungi.

	ACKNOWLEDGMENTS

We thank Richard van der Helm for providing a dimerum acid standard and useful discussions and Donald Nuss for providing plasmidpCPGHY1.

We thank the Maryland Agriculture Experiment Station for partialsupport.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Cell Biology & Molecular Genetics, University of Maryland, College Park,MD 20742-5815. Phone: (301) 405-1622. Fax: (301) 314-9082. E-mail:Straney{at}umail.umd.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Anke, T., and H. Diekmann. 1974. Incorporation of delta-N-hydroxy-L-ornithine and delta-N-acyl-delta-N-hydroxy-L-ornithine into sideramines of fungi. Arch. Microbiol. 95:227-236[CrossRef].

2. Atkin, C. L., J. B. Neilands, and H. J. Phaff. 1970. Rhodotorulic acid from species of Leucosporidium, Rhodosporidium, Rhodotorula, Sporidiobolus, and Sporobolomyces, and a new alanine-containing ferrichrome from Cryptococcus melibiosum. J. Bacteriol. 103:722-733[Abstract/Free Full Text].

3. Burt, W. R. 1982. Identification of coprogen B and its breakdown products from Histoplasma capsulatum. Infect. Immun. 35:990-996[Abstract/Free Full Text].

4. Buysens, S., K. Heungens, J. Poppe, and M. Hofte. 1996. Involvement of pyochelin and pyoverdin in suppression of Pythium-induced damping-off of tomato by Pseudomonas aeruginosa NSK2. Appl. Environ. Microbiol. 62:865-871[Abstract].

5. Choi, G., and D. Nuss. 1990. Nucleotide sequence of the glyceraldehyde-3-phosphate dehydrogenase gene from Cryphonectria parasitica. Nucleic Acids Res. 18:5566[Free Full Text].

6. Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Biochemistry 162:156-159.

7. Cook, R. J., and K. F. Baker. 1983. The nature and practice of biological control of plant pathogens. American Phytopathological Society, St. Paul, Minn.

8. Costa, J., and J. Loper. 1994. Characterization of siderophore production by the biological control agent Enterobacter cloacae. Mol. Plant-Microbe Interact. 7:440-448.

9. De Silva, A., K. Patterson, C. Rothrock, and J. Moore. 2000. Growth promotion of highbush blueberry by fungal and bacterial inoculants. HortScience 35:1228-1230[Abstract/Free Full Text].

10. Dori, S., Z. Solel, Y. Kashman, and I. Barash. 1990. Characterization of hydroxamate siderophores and siderophore-mediated iron uptake in Gaeumannomyces graminis var. tritici. Physiol. Mol. Plant Pathol. 37:95-106.

11. Duijff, B. J., A. H. M. Bakker, and B. Schippers. 1994. Suppression of fusarium wilt of carnation by Pseudomonas putida WCS358 at different levels of disease incidence and iron availability. Biocontrol Sci. Technol. 4:279-288.

12. Haese, A., M. Schubert, M. Herrmann, and R. Zocher. 1993. Molecular characterization of the enniatin synthetase gene encoding a multifunctional enzyme catalysing N-methyldepsipeptide formation in Fusarium scirpi. Mol. Microbiol. 7:905-914[Medline].

13. Harrington, G. J., and J. B. Neilands. 1982. Isolation and characterization of dimerum acid from Verticillium dahliae, a fungal phytopathogen, p. 675-682. In S. D. Nelson (ed.), Iron nutrition and interactions in plants. Marcel Dekker, New York, N.Y.

14. Hördt, W., V. Römheld, and G. Winkelmann. 2000. Fusarinines and dimerum acid, mono- and dihydroxamate siderophores from Penicillium chrysogenum, improve iron utilization by strategy I and strategy II plants. Biometals 13:37-46[CrossRef][Medline].

15. Hoskins, J., N. O'Callaghan, S. Queener, C. Cantwell, J. Wood, V. Chen, and P. Skatrud. 1990. Gene disruption of the pcbAB gene encoding ACV synthetase in Cephalosporium acremonium. Curr. Genet. 18:523-530[CrossRef][Medline].

16. Howard, D., R. Rafie, A. Tiwari, and K. Faull. 2000. Hydroxamate siderophores of Histoplasma capsulatum. Infect. Immun. 68:2338-2343[Abstract/Free Full Text].

17. Howell, C. R. 1987. Relevance of mycoparasitism in the biological control of Rhizoctonia solani by Gliocladium virens. Phytopathology 77:992-994.

18. Jalal, M. A., S. K. Love, and D. van der Helm. 1986. Siderophore mediated iron(III) uptake in Gliocladium virens. 1. Properties of cis-fusarinine, trans-fusarinine, dimerum acid, and their ferric complexes. J. Inorg. Biochem. 28:417-430[CrossRef][Medline].

19. Kirby, G. W., G. L. Patrick, and D. J. Robins. 1978. Cyclo-(L-phenyl-L-seryl) as an intermediate in the biosynthesis of gliotoxin. J. Chem. Soc. Trans. I 11:1336-1338.

20. Kleinkauf, H., and H. Von Dohren. 1996. A nonribosomal system of peptide biosynthesis. Eur. J. Biochem. 236:335-351[Medline].

21. Kraus, J., and J. E. Loper. 1992. Lack of evidence for a role of antifungal metabolite production by Pseudomonas fluorescens Pf-5 in biological control of pythium damping-off of cucumber. Phytopathology 82:264-271.

22. Leong, S. A., and G. Winkelmann. 1998. Molecular biology of iron transport in fungi. Met. Ions Biol. Syst. 35:147-186[Medline].

23. Loper, J. E., and J. S. Buyer. 1991. Siderophores in microbial interactions on plant surfaces. Mol. Plant-Microbe Interact. 4:5-13.

24. Lumsden, R. D., and J. C. Locke. 1989. Biological control of damping-off caused by Pythium ultimum and Rhizoctonia solani with Gliocladium virens in soilless mix. Phytopathology 79:361-366.

25. Lumsden, R. D., J. C. Locke, S. T. Adkins, J. F. Walter, and C. J. Ridout. 1992. Isolation and localization of the antibiotic gliotoxin produced by Gliocladium virens from alginate prill in soil and soilless media. Phytopathology 82:230-235.

26. Lumsden, R. D., J. F. Walter, and C. P. Baker. 1996. Development of Gliocladium virens for damping-off disease control. Can. J. Plant Pathol. 18:463-468.

27. Ongena, M., F. Daayf, P. Jacques, P. Thonart, P. Thonart, N. Benhamou, T. C. Paulitz, P. Cornelis, N. Koedam, and R. R. Belanger. 1998. Protection of cucumber against Pythium root rot by fluorescent pseudomonads: predominant role of induced resistance over siderophores antibiosis. Plant Pathol. 48:66-76[CrossRef].

28. Ownley, B., D. Weller, and L. Thomashow. 1992. Influence of in situ and in vitro pH on suppression of Gaeumannomyces graminis var. tritici by Pseudomonas fluorescens 2-79. Phytopathology 82:178-184.

29. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

30. Samuels, G. J., and S. A. Rehner. 1993. Toward a concept of genus and species in Trichoderma, p. 186-188. In R. D. Lumsden, and J. L. Vaughn (ed.), Pest management: biologically based technologies. American Chemical Society, Washington, D.C.

31. Scott-Craig, J. S., D. G. Panaccione, J. A. Pocard, and J. D. Walton. 1992. The cyclic peptide synthetase catalyzing HC-toxin production in the filamentous fungus Cochliobolus carbonum is encoded by a 15.7-kilobase open reading frame. J. Biol. Chem. 267:26044-26049[Abstract/Free Full Text].

32. Stachelhaus, T., and M. Marahiel. 1995. Modular structure of genes encoding multifunctional peptide synthetases required for non-ribosomal peptide synthesis. FEMS Microbiol. Lett. 125:3-14[CrossRef][Medline].

33. Thomas, M. D., and C. M. Kenerley. 1989. Transformation of the mycoparasite Gliocladium. Curr. Genet. 15:415-420[CrossRef].

34. Turgay, K., M. Krause, and M. Marahiel. 1992. Four homologous domains in the primary structure of GrsB are related to domains in a superfamily of adenylate-forming enzymes. Mol. Microbiol. 6:529-546[Medline].

35. Turgeon, G. B., R. C. Garber, and O. C. Yoder. 1985. Transformation of the fungal maize pathogen Cocliobolus heterostrophus using the Aspergillus nidulans amdS gene. Mol. Gen. Genet. 201:450-453[CrossRef].

36. von Döhren, H., U. Keller, J. Vater, and R. Zocher. 1997. Multifunctional peptide synthetases. Chem. Rev. 97:2675-2705[CrossRef][Medline].

37. Wilhite, S. E., R. D. Lumsden, and D. C. Straney. 1994. Mutational analysis of gliotoxin production by the biocontrol fungus Gliocladium virens in relation to suppression of pythium damping-off. Phytopathology 84:816-821.

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1.	Anke, T., and H. Diekmann. 1974. Incorporation of delta-N-hydroxy-L-ornithine and delta-N-acyl-delta-N-hydroxy-L-ornithine into sideramines of fungi. Arch. Microbiol. 95:227-236[CrossRef].
2.	Atkin, C. L., J. B. Neilands, and H. J. Phaff. 1970. Rhodotorulic acid from species of Leucosporidium, Rhodosporidium, Rhodotorula, Sporidiobolus, and Sporobolomyces, and a new alanine-containing ferrichrome from Cryptococcus melibiosum. J. Bacteriol. 103:722-733[Abstract/Free Full Text].
3.	Burt, W. R. 1982. Identification of coprogen B and its breakdown products from Histoplasma capsulatum. Infect. Immun. 35:990-996[Abstract/Free Full Text].
4.	Buysens, S., K. Heungens, J. Poppe, and M. Hofte. 1996. Involvement of pyochelin and pyoverdin in suppression of Pythium-induced damping-off of tomato by Pseudomonas aeruginosa NSK2. Appl. Environ. Microbiol. 62:865-871[Abstract].
5.	Choi, G., and D. Nuss. 1990. Nucleotide sequence of the glyceraldehyde-3-phosphate dehydrogenase gene from Cryphonectria parasitica. Nucleic Acids Res. 18:5566[Free Full Text].
6.	Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Biochemistry 162:156-159.
7.	Cook, R. J., and K. F. Baker. 1983. The nature and practice of biological control of plant pathogens. American Phytopathological Society, St. Paul, Minn.
8.	Costa, J., and J. Loper. 1994. Characterization of siderophore production by the biological control agent Enterobacter cloacae. Mol. Plant-Microbe Interact. 7:440-448.
9.	De Silva, A., K. Patterson, C. Rothrock, and J. Moore. 2000. Growth promotion of highbush blueberry by fungal and bacterial inoculants. HortScience 35:1228-1230[Abstract/Free Full Text].
10.	Dori, S., Z. Solel, Y. Kashman, and I. Barash. 1990. Characterization of hydroxamate siderophores and siderophore-mediated iron uptake in Gaeumannomyces graminis var. tritici. Physiol. Mol. Plant Pathol. 37:95-106.
11.	Duijff, B. J., A. H. M. Bakker, and B. Schippers. 1994. Suppression of fusarium wilt of carnation by Pseudomonas putida WCS358 at different levels of disease incidence and iron availability. Biocontrol Sci. Technol. 4:279-288.
12.	Haese, A., M. Schubert, M. Herrmann, and R. Zocher. 1993. Molecular characterization of the enniatin synthetase gene encoding a multifunctional enzyme catalysing N-methyldepsipeptide formation in Fusarium scirpi. Mol. Microbiol. 7:905-914[Medline].
13.	Harrington, G. J., and J. B. Neilands. 1982. Isolation and characterization of dimerum acid from Verticillium dahliae, a fungal phytopathogen, p. 675-682. In S. D. Nelson (ed.), Iron nutrition and interactions in plants. Marcel Dekker, New York, N.Y.
14.	Hördt, W., V. Römheld, and G. Winkelmann. 2000. Fusarinines and dimerum acid, mono- and dihydroxamate siderophores from Penicillium chrysogenum, improve iron utilization by strategy I and strategy II plants. Biometals 13:37-46[CrossRef][Medline].
15.	Hoskins, J., N. O'Callaghan, S. Queener, C. Cantwell, J. Wood, V. Chen, and P. Skatrud. 1990. Gene disruption of the pcbAB gene encoding ACV synthetase in Cephalosporium acremonium. Curr. Genet. 18:523-530[CrossRef][Medline].
16.	Howard, D., R. Rafie, A. Tiwari, and K. Faull. 2000. Hydroxamate siderophores of Histoplasma capsulatum. Infect. Immun. 68:2338-2343[Abstract/Free Full Text].
17.	Howell, C. R. 1987. Relevance of mycoparasitism in the biological control of Rhizoctonia solani by Gliocladium virens. Phytopathology 77:992-994.
18.	Jalal, M. A., S. K. Love, and D. van der Helm. 1986. Siderophore mediated iron(III) uptake in Gliocladium virens. 1. Properties of cis-fusarinine, trans-fusarinine, dimerum acid, and their ferric complexes. J. Inorg. Biochem. 28:417-430[CrossRef][Medline].
19.	Kirby, G. W., G. L. Patrick, and D. J. Robins. 1978. Cyclo-(L-phenyl-L-seryl) as an intermediate in the biosynthesis of gliotoxin. J. Chem. Soc. Trans. I 11:1336-1338.
20.	Kleinkauf, H., and H. Von Dohren. 1996. A nonribosomal system of peptide biosynthesis. Eur. J. Biochem. 236:335-351[Medline].
21.	Kraus, J., and J. E. Loper. 1992. Lack of evidence for a role of antifungal metabolite production by Pseudomonas fluorescens Pf-5 in biological control of pythium damping-off of cucumber. Phytopathology 82:264-271.
22.	Leong, S. A., and G. Winkelmann. 1998. Molecular biology of iron transport in fungi. Met. Ions Biol. Syst. 35:147-186[Medline].
23.	Loper, J. E., and J. S. Buyer. 1991. Siderophores in microbial interactions on plant surfaces. Mol. Plant-Microbe Interact. 4:5-13.
24.	Lumsden, R. D., and J. C. Locke. 1989. Biological control of damping-off caused by Pythium ultimum and Rhizoctonia solani with Gliocladium virens in soilless mix. Phytopathology 79:361-366.
25.	Lumsden, R. D., J. C. Locke, S. T. Adkins, J. F. Walter, and C. J. Ridout. 1992. Isolation and localization of the antibiotic gliotoxin produced by Gliocladium virens from alginate prill in soil and soilless media. Phytopathology 82:230-235.
26.	Lumsden, R. D., J. F. Walter, and C. P. Baker. 1996. Development of Gliocladium virens for damping-off disease control. Can. J. Plant Pathol. 18:463-468.
27.	Ongena, M., F. Daayf, P. Jacques, P. Thonart, P. Thonart, N. Benhamou, T. C. Paulitz, P. Cornelis, N. Koedam, and R. R. Belanger. 1998. Protection of cucumber against Pythium root rot by fluorescent pseudomonads: predominant role of induced resistance over siderophores antibiosis. Plant Pathol. 48:66-76[CrossRef].
28.	Ownley, B., D. Weller, and L. Thomashow. 1992. Influence of in situ and in vitro pH on suppression of Gaeumannomyces graminis var. tritici by Pseudomonas fluorescens 2-79. Phytopathology 82:178-184.
29.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
30.	Samuels, G. J., and S. A. Rehner. 1993. Toward a concept of genus and species in Trichoderma, p. 186-188. In R. D. Lumsden, and J. L. Vaughn (ed.), Pest management: biologically based technologies. American Chemical Society, Washington, D.C.
31.	Scott-Craig, J. S., D. G. Panaccione, J. A. Pocard, and J. D. Walton. 1992. The cyclic peptide synthetase catalyzing HC-toxin production in the filamentous fungus Cochliobolus carbonum is encoded by a 15.7-kilobase open reading frame. J. Biol. Chem. 267:26044-26049[Abstract/Free Full Text].
32.	Stachelhaus, T., and M. Marahiel. 1995. Modular structure of genes encoding multifunctional peptide synthetases required for non-ribosomal peptide synthesis. FEMS Microbiol. Lett. 125:3-14[CrossRef][Medline].
33.	Thomas, M. D., and C. M. Kenerley. 1989. Transformation of the mycoparasite Gliocladium. Curr. Genet. 15:415-420[CrossRef].
34.	Turgay, K., M. Krause, and M. Marahiel. 1992. Four homologous domains in the primary structure of GrsB are related to domains in a superfamily of adenylate-forming enzymes. Mol. Microbiol. 6:529-546[Medline].
35.	Turgeon, G. B., R. C. Garber, and O. C. Yoder. 1985. Transformation of the fungal maize pathogen Cocliobolus heterostrophus using the Aspergillus nidulans amdS gene. Mol. Gen. Genet. 201:450-453[CrossRef].
36.	von Döhren, H., U. Keller, J. Vater, and R. Zocher. 1997. Multifunctional peptide synthetases. Chem. Rev. 97:2675-2705[CrossRef][Medline].
37.	Wilhite, S. E., R. D. Lumsden, and D. C. Straney. 1994. Mutational analysis of gliotoxin production by the biocontrol fungus Gliocladium virens in relation to suppression of pythium damping-off. Phytopathology 84:816-821.