Characterization of a Novel, Antifungal, Chitin-Binding Protein from Streptomyces tendae Tu901 That Interferes with Growth Polarity

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Journal of Bacteriology, December 1999, p. 7421-7429, Vol. 181, No. 24
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Characterization of a Novel, Antifungal, Chitin-Binding Protein from Streptomyces tendae Tü901 That Interferes with Growth Polarity

Christiane Bormann,¹^,^* Daniel Baier,¹ Ingmar Hörr,² Claudia Raps,¹ Jürgen Berger,³ Günther Jung,² and Heinz Schwarz³

Mikrobiologie/Biotechnologie¹ and Organische Chemie,² Universität Tübingen, and Max-Planck-Institut für Entwicklungsbiologie,³ D-72076 Tübingen, Germany

Received 3 August 1999/Accepted 27 September 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The afp1 gene, which encodes the antifungal protein AFP1, was cloned from nikkomycin-producing Streptomyces tendae Tü901,using a nikkomycin-negative mutant as a host and screening transformantsfor antifungal activity against Paecilomyces variotii in agardiffusion assays. The 384-bp afp1 gene has a low G+C content (63%)and a transcription termination structure with a poly(T) region,unusual attributes for Streptomyces genes. AFP1 was purified fromculture filtrate of S. tendae carrying the afp1 gene on the multicopyplasmid pIJ699. The purified protein had a molecular mass of 9,862Da and lacked a 42-residue N-terminal peptide deduced from thenucleotide sequence. AFP1 was stable at extreme pH values andhigh temperatures and toward commercial proteinases. AFP1 hadlimited similarity to cellulose-binding domains of microbial plantcell wall hydrolases and bound to crab shell chitin, chitosan,and cell walls of P. variotii but showed no enzyme activity. Thebiological activity of AFP1, which represents the first chitin-bindingprotein from bacteria exhibiting antifungal activity, was directedagainst specific ascomycetes, and synergistic interaction withthe chitin synthetase inhibitor nikkomycin inhibited growth ofAspergillus species. Microscopy studies revealed that fluorescein-labeledAFP1 strongly bound to the surface of germinated conidia and totips of growing hyphae, causing severe alterations in cell morphogenesisthat gave rise to large spherical conidia and/or swollen hyphaeand to atypicalbranching.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Proteins with antifungal activity have been isolated from plants, insects, and fungi and characterized. Plant antifungal proteins,including the cysteine-rich small defensins, ribosome-inactivatingproteins, lipid transfer proteins, polygalacturonase inhibitorproteins, nonenzymatic chitin-binding proteins, and pathogenesis-related(PR) proteins, appear to comprise defense mechanisms against fungalattack (54). Many of these proteins are rapidly induced uponinfection with fungal, bacterial, viral, or viroidal pathogensor by related forms of stress. Among the induced proteins arethe PR proteins, which have been classified into families basedon amino acid sequence similarities, serological properties, andfunction (22, 24, 43). Members of the five major families(1 to 5) have been shown to have in vitro antifungal activities.PR proteins of families 2 and 3 (PR-2 and PR-3 proteins) include $beta$ -1,3-glucanases and chitinases, respectively, which act synergisticallyin degrading fungal cell walls and inhibit growth of fungi. Manyof the PR-4 proteins have nonenzymatic chitin-binding activity,and PR-5 proteins are related to salt-induced osmotins, whichhave been shown to permeabilize the fungal plasma membrane andinhibit spore germination and hyphal growth (1, 47, 51).A small histidine-rich antifungal protein and cysteine-rich antifungalproteins have been isolated from insects (8, 20). The latterproteins, which have significant sequence similarity to the 5-kDaplant defensins, inhibit spore germination and cause partial lysisof fungal hyphae. Small, highly basic, and cysteine-rich antifungalproteins not related to plant antifungal proteins have been purifiedfrom the extracellular medium of some imperfect ascomycetes (25,31). These proteins reveal some sequence similarity to phospholipaseA₂, but their molecular mode of action is notknown.

Antifungal proteins are of great biotechnological interest because of their potential use as food and seed preservative agentsand for engineering plants for resistance to phytopathogenic fungi(6). Various studies have revealed that transgenic plants overexpressinggenes of the PR-1, PR-2, PR-3, and PR-5 families mediate hostplant resistance to phytopathogenic fungi, and coexpression ofmultiple antifungal protein genes in transgenic plants seems tobe more effective than expression of single genes (for a review,see reference 54).

Antifungal proteins have not yet been isolated from streptomycetes and other bacteria. Streptomycetes are gram-positive, mycelium-formingsoil bacteria that have the capacity to produce a great varietyof secreted proteins, including hydrolytic enzymes that degradeorganic material in the soil, such as chitin, cellulose, xylan,and starch (33), and enzyme inhibitors (7, 14, 30). Furthermore,streptomycetes have the exceptional ability to produce a broadrange of low-molecular-weight antibiotics and other secondarymetabolites; many of these compounds have antibacterial and antifungalproperties and are used as agents in medicine and agriculture.Streptomyces tendae Tü901 produces antibiotics of various chemicalstructures, including cyclohexenylglycine, an isoleucine antagonistwith antibacterial activity (23); the naphthoquinone compoundjuglomycin, which has antitumor activity (11); and chlorothricin,a glycosylated macrolide antibiotic that acts as an antagonistof acetyl-coenzyme A in bacteria (9). In addition, the strainsynthesizes various nikkomycins, which are peptidyl nucleosideantibiotics. Nikkomycins act as specific inhibitors of chitinsynthetases and have high antifungal, insecticidal, and acaricidalactivity (for a review, see reference 12).

In an attempt to isolate nikkomycin biosynthesis genes, we transformed a nikkomycin-nonproducing mutant of S. tendae Tü901with DNA fragments from S. tendae Tü901 cloned into the multicopyplasmid pIJ699 and screened for antifungally active transformants,using Paecilomyces variotii as the test organism. In the courseof these experiments, we cloned a gene for a protein that exhibitsantifungal activity. Here, we present the characterization ofthis antifungal protein, AFP1, and its gene and show that AFP1is a chitin-binding protein that strongly binds to the cell wallof germinated conidia and to hyphal tips of sensitive fungi andinterferes with their growthpolarity.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Microorganisms and plasmids. S. tendae Tü901/8c, which produces nikkomycins I, J, X, and Z, was obtained from H. Zähner, University of Tübingen, Tübingen,Germany. S. tendae Tü901/NP51 is a nonproducing mutant of S.tendae Tü901/8c which does not synthesize antifungally activenikkomycins (4). S. lividans TK23 was obtained from D. A. Hopwood,John Innes Institute, Norwich, England. Plasmids pIJ699 (21)and pIJ486 (49) were provided by T. Kieser and D. A. Hopwood,John Innes Institute, and were used for cloning in Streptomyces.Escherichia coli JM83 {F ara $Delta$ (lac-proAB) rpsL(Str^r) [ $phi$ 80dlac $Delta$ (lacZ)M15]thi} and vectors pUC18/19 (53) were usedfor subcloning. The plasmids constructed for use in this studyare shown in Fig. 1.

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FIG. 1. Restriction map of the 14.5-kb BamHI insert of pAE11 and subcloned fragments containing the afp1 gene. Bold lines represent segments of the vector pIJ699. The nucleotide sequence of the 2.08-kb BamHI-XbaI insert of pUCK12 was determined. The size and location of the afp1 gene and the 5' region of orf2 were deduced from the nucleotide sequence and are indicated by an arrow and a box, respectively. Abbreviations for restriction enzymes: B, BamHI; Bg, BglII; H, HindIII; K, KpnI; X, XhoI; Xb, XbaI.

Test organisms for the determination of biological activity of AFP1 were E. coli DSM 498 (strain K-12), Micrococcus luteusDSM 1790, Candida albicans Tü167, Yarrowia lipolytica DSM 70562,Saccharomyces cerevisiae Tü125, Mucor miehei Tü284, Mucor hiemalisTü179, Aspergillus terreus, Aspergillus fumigatus Tü161, Aspergillusniger Tü504, Cladosporium herbarum DSM 63422, Mycotypha africanaDSM 3118, P. variotii Tü137, Penicillium chrysogenum DSM 844,and Trichophyton mentagrophytes Tü510 and were obtained fromthe culture collection of the Institute of Microbiology I, Universityof Tübingen (Tü strains) or from the Deutsche Sammlung von Mikroorganismenund Zellkulturen GmbH (DSMZstrains).

Culture conditions. S. tendae NP51(pK11) and S. lividans(pK112) were grown on solid HA medium (3) containing 30 µg of thiostrepton ml¹ at 27°C. Liquid cultures were incubated on a rotatory shakerat 27°C as described previously (27), and AFP1 production wasmonitored on nikkomycin production medium SP (27), modifiedprecultivation CRM medium, and HA medium (3). These media werebuffered by 50 or 100 mM MES (2-[N-morpholino]ethanesulfonic acid),pH 6.0. Thiostrepton (Sigma) was added at a concentration of 10µg ml¹ to liquid media. Agar diffusion assays with fungi and bacteriaas test organisms were done on HA agar at pH 6.0 and 7.0, respectively.Malt extract peptone agar (3% malt extract, 0.3% soy peptone,1.5% agar [pH 5.6]) was used for cultivation of C. herbarum andT. mentagrophyta.

Manipulation of DNA and cloning procedures. Standard procedures were used for E. coli (38). Total DNA from S. tendae Tü901/8c was isolated by a large-scale method(19), and plasmid DNA was isolated by the alkaline lysis method(18). Streptomyces protoplasts were transformed as describedby Bormann et al. (3).

For genetic complementation experiments, total DNA from S. tendae Tü901/8c was partially digested with BamHI, and the resultingfragments were size fractionated. Fragments of 15 to 25 kb wereligated to BglII-cleaved pIJ699 isolated from S. tendae Tü901/8c.S. tendae Tü901/NP51 was transformed with the ligation mixture,and the resulting thiostrepton-resistant transformants were grownin 10-mm² patches on solid HA medium for 5 days. Agar plugs (6 mm in diameter)containing transformants were cut and placed onto test plateswith P. variotii as the testfungus.

DNA sequencing. The nucleotide sequence was determined by the dideoxy chain termination method using a T7 sequencing kit, deaza-dGTP reactionmixtures, [ $alpha$ -³⁵S]dATP (Amersham Pharmacia Biotech Europe GmbH), and pUCK12 andsubclones in pUC vectors with the M13/pUC universal and reverseprimers. The CODONPREFERENCE program of the University of WisconsinGenetics Computer Group package and the PC/GENE software package(IntelliGenetics) were used for sequence analysis. Databases weresearched by using the program $Psi$ -BLAST (release 36) (2).

Purification and characterization of AFP1 protein. Culture filtrate (200 ml) from S. tendae NP51(pK11) grown for 5 days in CRM medium was adjusted to pH 3.0 with 1 M HCl andstirred for 1 h at 4°C. Denatured proteins were precipitated bycentrifugation at 10,000 × g for 30 min. The supernatant was desaltedand buffered to 25 mM sodium acetate (pH 3.0) by chromatographyon a Sephadex G-25 medium (Amersham Pharmacia Biotech) column(5 by 20 cm) previously equilibrated with the same buffer at aflow rate of 5 ml min¹. AFP1-containing fractions were fractionated on an S-Sepharosecolumn (HR 16/10; Pharmacia) previously equilibrated with 25 mMsodium acetate buffer (pH 3.0) at a flow rate of 100 ml h¹. Most proteins did not bind to the resin. After elution of proteinsby 100 ml of 0.2 M NaCl in 25 mM sodium acetate buffer (pH 3.0),AFP1 was eluted by 0.3 M NaCl in the same buffer. AFP1-containingfractions were collected, desalted by passage through SephadexG-25 PD-10 columns (Amersham Pharmacia Biotech), andlyophilized.

AFP1 activity was determined by agar diffusion assays using P. variotii as the test organism calibrated with purified AFP1(4 to 30 µg; Fig. 5).

The Stokes radius of purified AFP1 (100 µg) was determined by gel filtration chromatography on a Superose 12 column (HR 10/30;Amersham Pharmacia Biotech) equilibrated with 25 mM Tris-HCl buffer(pH 7)-0.1 M NaCl at a flow rate of 0.5 ml min¹. Reference proteins (Sigma) were insulin $beta$ chain (3,495.9 Da),cytochrome c (12,327 Da), carbonic anhydrase (29,000 Da), alcoholdehydrogenase from yeast (150,000 Da), and sweet potato $beta$ -amylase(200,000 Da). The molecular mass was also determined by electrospraymass spectrometry on an API III triple-quadrupole mass spectrometer(Sciex, Thornhill,Canada).

The N-terminal sequence of purified AFP1 was determined by automated Edman degradation in a pulse-liquid protein sequencer477A (Applied Biosystems) equipped with an online analyzer 120A(Applied Biosystems) for phenylthiohydantoin-derivatized aminoacids.

Determination of cysteine by using Ellmann's reagent. To test for cysteine and cystine residues in AFP1, the reaction with Ellmann's reagent was carried out before and after treatmentwith sodium borohydride (17). AFP1 (20 or 40 µg in 45 µl) wasincubated in the presence or absence of 2.5% sodium borohydridein water at 50°C for 1 h. After destruction of the remaining borohydrideby addition of 20 µl of 1 N HCl and incubation for 30 min at roomtemperature, 25-µl aliquots of each sample were removed and usedfor agar diffusion assays with P. variotii as the test organism;200 µl of Ellmann's reagent [0.05% 5,5'-dithio-bis(5-nitrobenzoicacid) (Sigma) in 0.22 M Tris-HCl, pH 8.2] was added to the remainingsamples. After incubation for 5 min at room temperature, the absorbanceat 412 nm was measured. Absorbances of the reduced AFP1 solutions(20 µg of AFP1 and 40 µg of AFP1) were 0.074 and 0.148, respectively;the absorbance of the native protein (40 µg) was 0.002. Inhibitionzones toward P. variotii were not obtained for NaBH₄-treated samples,while untreated AFP1 samples gave inhibition zones 12 and 14 mmindiameter.

Determination of stability. Temperature stability was investigated by incubating purified AFP1 (1 mg ml¹ in 25 mM MES-NaOH (pH 6) in sealed vessels at 40 to 100°C. Samples(20 µl) were removed between 0 and 60 min. pH stability of purifiedAFP1 (1 mg ml¹) was investigated at pH 1.5 to 12 at 4 and 24°C. Samples (20µl) were taken after 0, 1, 2, 3, 4, 5, and 8 days. The followingbuffers (25 mM) were used: glycine-HCl, pH 1.5 and 2; sodium acetate-NaOH,pH 3; citric acid-Na₂HPO₄, pH 4 and 5; MES-NaOH, pH 6; TES (N-tris[hydroxymethyl]methyl-2-aminoethanesulfonicacid)-NaOH, pH 7; HEPES-NaOH, pH 8; TAPS (N-tris[hydroxymethyl]methyl-3-aminopropanesulfonicacid)-NaOH, pH 9; and glycine-NaOH, pH 10, 11, and 12. Stabilitytoward proteases was assayed by incubating 7 µg of AFP1 and 10µg of pepsin, proteinase K, pronase, or trypsin (all from Sigma)in 0.1 M citric acid-0.2 M Na₂PO₄ (at pH 4 and 5 for pepsin andat pH 7 for the other enzymes) for 3 and 12 h at 37°C. Antifungalactivity of the samples was determined by agar diffusion assaysusing P. variotii as the testorganism.

PAGE. Proteins were separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) on 16% polyacrylamide gelscontaining 6 M urea in the Tris-Tricine (N-tris[hydroxymethyl]glycine)buffer system described by Schägger and von Jagow (39), whichallowed a good separation of proteins with molecular masses of<10 kDa. Prestained molecular mass standards (Gibco BRL, LifeTechnologies) were insulin $alpha$ and $beta$ chain (3,000 Da), bovine trypsininhibitor (6,200 Da), lysozyme (14,300 Da), $beta$ -lactoglobulin (18,400Da), carbonic anhydrase (29,000 Da), and ovalbumin (43,000 Da).Proteins in gels were detected by staining with Coomassie blueG250.

Determination of antifungal activity. Agar diffusion assays were performed to determine the antifungal activity of AFP1-containing agar or solutions and to characterizethe spectrum of biological activity of AFP1. Test plates (85 mmin diameter) contained 17.5 ml of HA agar seeded with test organisms,either spores of filamentous fungi or cells of bacteria and yeastsgrown overnight in liquid HA medium, at a concentration of (10⁵). AFP1-containing solutions were applied to paper disks (6 mmin diameter) or in wells (6 mm in diameter) punched into the agar.Test plates were incubated for at least 24 h at 37°C for E. coli,M. miehei, A. fumigatus, and P. variotii, at 24°C for C. herbarum,and at 27°C for the remaining test organisms. All results deducedfrom agar diffusion assays were calculated from three independentexperiments. To assay for inhibition of hyphal growth, an agarplug containing mycelia of the test fungus was placed in the centerof a petri dish containing 17.5 ml of HA agar and incubated untilthe colony reached a diameter of 3 to 4 cm. A paper disk containing20 or 30 µg of AFP1 was placed at the growing front of the hyphae,and the test plates were incubatedfurther.

High-pressure liquid chromatography (HPLC) analysis was used to check culture filtrates for nikkomycins (10).

Labeling of AFP1. AFP1 (1 mg) was labeled with 0.236 mg of 5(6)-carboxyfluorescein-N-hydroxysuccinimide ester according to the specificationsof the fluorescein labeling kit supplied by Boehringer (Mannheim,Germany).

Assays. Chitin azur (Sigma), p-nitrophenyl $beta$ -D-N,N',N"-triacetylchitotriose (Sigma), laminarin (Sigma), and whole mycelia of P. variotiiwere used as substrates to assay AFP1 for chitinase, $beta$ -1,3-glucanase,and cell wall-degrading activity, respectively. P. variotii myceliagrown in liquid HA medium were homogenized in an Ultraturrax blenderfor 15 s. Cell debris was sedimented by centrifugation at 20,000× g for 20 min, washed three times with deionized water, lyophilized,and used for estimation of sugar liberation. The reaction mixtureconsisted of 0.5 ml of substrate suspension (4 mg ml¹) in 0.1 M citric acid-0.2 M Na₂HPO₄ buffer (pH 7) or in 0.1 Mammonia acetate buffer (pH 5) and 0.1 ml of AFP1 (50 µg in distilledwater) and was incubated at 37°C with shaking for 12 to 48 h.Undissolved substrates were removed by centrifugation. Degradationof chitin azur was determined by measuring the absorbance at 570nm. The amount of reduced sugars released from laminarin or fungalmycelia was assayed with the low-alkalinity copper reagent ofSomogyi (41) and arsenomolybdate chromogen of Nelson (32).With p-nitrophenyl $beta$ -D-N,N',N"-triacetylchitotriose as the substrate,the reaction mixture consisted of 0.12 ml of substrate (2 mg ml¹) in 0.1 M citric acid-0.2 M Na₂HPO₄ buffer (pH 7.0) and 100 µgof AFP1. After incubation for 4 h at 37°C, absorbance was determinedat 410 nm. Positive control reactions were performed with chitinasefrom S. griseus (Sigma) and laminarinase from mollusk(Sigma).

Binding assays were performed with Avicel PH-101 (Fluka BioChemika), xylan from birchwood (Sigma), curdlan from Alcaligenesfaecalis (Sigma), purified crab shell chitin (Sigma), chitosanfrom crab shells (Sigma), and cell walls of P. variotii. Fluoresceinisothiocyanate (FITC)-labeled AFP1 (10 µg) was incubated with5 mg of polyglycan and 1 mg of cell walls in 100 µl of 100 mMTris-HCl (pH 7.6) overnight on a rotator. After three washes withthe same buffer containing 150 mM NaCl, the samples were inspectedbymicroscopy.

Microscopy. For fluorescence microscopy, samples were mounted in 16.7% (wt/vol) Moviol (Hoechst)-33.3% (vol/vol) glycerol in 66.7 mM Tris-HCl(pH 8 (37). A Zeiss Axiophot 2 microscope, the FITC filter tovisualize FITC-labeled AFP1, and Kodak T-Max films (ASA 100 andASA 1000) were used forphotographs.

Nucleotide accession number. The nucleotide sequence data described in this report have been deposited at the EMBL nucleotide sequence database under accessionno. AJ242827.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Cloning of the AFP1-encoding gene. The mutant S. tendae Tü901/NP51, which does not synthesize biologically active nikkomycins (4), was transformed with agenomic library of S. tendae Tü901 in pIJ699, constructed asdescribed in Materials and Methods. To screen for antifungallyactive transformants, agar plugs containing thiostrepton-resistanttransformants grown in patches on complex agar medium were cutand incubated on plates containing spores of P. variotii. Amongapproximately 2,000 transformants, one caused a clear zone ofgrowth inhibition about 10 mm in diameter. The recombinant plasmidpAE11 isolated from this transformant carried a 14.5-kb insert(Fig. 1). When pAE11 was reintroduced into mutant NP51, about70% of the new transformants grown on solid medium caused zonesof growth inhibition of P. variotii.

The antifungal activity of the transformants was obviously not derived from genetic complementation of mutant NP51 to nikkomycinsynthesis since nikkomycins (at concentrations >3 mg/liter) werenot detected by HPLC of culture filtrates of transformants grownin nikkomycin production medium. Furthermore, when the culturefiltrate was passed through a membrane filter with an exclusionlimit of 10 kDa, which would not retain nikkomycins (approximately600 Da), the antifungally active compound was retained on thefilter. To localize the encoding gene, designated afp1 (antifungalprotein 1), subclones of pAE11 were constructed. The presenceof the deletion plasmid pK11, which lacked three KpnI fragmentsand contained a 2.8-kb insert, or plasmid pK112, which carriedthe 1.1-kb XhoI-BamHI fragment from pK11 (Fig. 1), led to expressionof the antifungal protein in S. tendae NP51 and S. lividansTK23.

DNA sequence analysis. The nucleotide sequence of the 2,087-bp BamHI-XbaI fragment cloned from pK11 into pUC19 (forming pUCK12) was determined andanalyzed. A complete open reading frame, afp1, composed of 384bp, and the 5' end of a putative second open reading frame, orf2,were identified (Fig. 1 and 2). The afp1 gene has two potentialATG start codons, at nucleotides (nt) 411 and 417; the latteris preceded by a potential ribosome-binding site (GAGG; nt 407to 410) and therefore is the proposed translational start site.The afp1 gene terminates at a TGA stop codon at nt 801 and couldencode a protein of 128 amino acids. The G+C content of the afp1gene is 63.3%, much lower than that of the total Streptomycesgenome (73%). The region upstream of the afp1 gene (nt 1 to 416)also has a low G+C content (60.7%). In the distal region of the3' end of the afp1 gene are found a 9-bp, GC-rich inverted repeatregion and an adjacent poly(I) region of 8 nt, which are rarefor potential Streptomyces transcription terminators. Databasesearches revealed limited sequence similarity (25 to 33% identity,41 to 53% similarity) between 40 to 77 amino acid residues ofAFP1 and N-acetylmuramoyl-L-alanine amidase from Synechocystissp., cellulase CelE from Pseudomonas fluorescens, and endo-1,4- $beta$ -xylanasesfrom Bacillus and Ruminococcus spp. (GenBank accession no. D90909,X86798, X59059, and U43089). The region of sequence similaritywithin CelE constitutes a part of the 100-amino-acid cellulose-bindingdomain, which is characterized by several highly conserved tryptophanresidues in addition to glycine and asparagine residues and thelack of charged amino acids (12a). The region of similarity betweenAFP1 and the xylanases is located in the catalytic domain of theenzymes. $Psi$ -Blast iterations revealed similarity between AFP1 andcellulose-binding domains of other cellodextrinases, xylanases,and esterase D from Pseudomonas fluorescens (Fig. 3) and to asequence in the catalytic domain of various xylanases.

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FIG. 2. Nucleotide sequence of the S. tendae Tü901 afp1 gene and the predicted amino acid sequence. A putative ribosome-binding site (SD) is overlined. The translational start site of the afp1 gene is indicated by an arrow, and the termination codon is marked by a dash. Amino acids determined experimentally by N-terminal sequencing are underlined. The proposed cleavage site for signal peptidase is in boldface. $right-arrow$ $left-arrow$ indicates an inverted repeat sequence, and the poly(T) region is underlined.

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FIG. 3. BLASTP sequence alignment of amino acid residues 3 to 75 of the extracellular AFP1 with segments of N-acetylmuramoyl-L-alanine amidase from Synechocystis sp. (AmiA) and cellulase CelE (CelE), endoglucanase A (EGA), cellodextrinase (EGC), xylanase A (XylA), and esterase D (EstD) from Pseudomonas fluorescens. The sequences were obtained from GenBank (AFP1, this work; CelE, X86798; AmiA, D90909; CelE, X86798; EGA, X12570; EstD, X15429), from the PIR database (EGC, S19652), and from Swiss-Prot (XylA, P14768). CBD indicates residues of cellulose-binding domains which are identical or similar in the aligned sequences of CelE, EGA, EGC, XylA, and EstD. Aromatic amino acid residues involved in protein-sugar binding (34) are boxed. Amino acid residues that are identical in six of seven sequences are in boldface.

The potential open reading frame orf2 could begin at the ATG start codon at nt 1249 or at nt 1285, each of which is precededby a potential ribosome-binding site (AGGG, nt 1239 to 1242; GGGA,nt 1279 to 1282). The corresponding incomplete orf2 has a G+Ccontent of 70.9%. The encoded N-terminal portion of the protein,composed of 277 or 266 amino acids, respectively, did not revealany similarity to protein sequences indatabases.

Purification of the AFP1 protein. To purify AFP1, S. tendae NP51 carrying pK11 was first cultivated in various media and culture filtrates were analyzed forantifungal activity by agar diffusion assays. Antifungal activitywas of a similar high value when SP or CRM medium was used. CRMmedium, which contains less proteinaceous compounds that couldinterfere with the purification procedure, was used for furtherexperiments. Culture filtrates were collected throughout the growthof S. tendae NP51(pK11) and assayed by agar diffusion tests andSDS-PAGE (Fig. 4). Antifungal activity of culture filtrates increasedto a maximum level corresponding to approximately 300 mg of AFP1liter¹ at 120 h in the stationary growth phase and remained constantwhen mycelia were cultivated for a further 24 h. SDS-PAGE analysisrevealed that AFP1 appeared as the major protein of antifungallyactive culture filtrates and migrated near the 5,000-Da markerprotein.

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FIG. 4. Time course of AFP1 production in S. tendae NP51(pK11) cultivated in CRM medium. (A) AFP1 (

) in the culture filtrate determined by agar diffusion assays with P. variotii as the test fungus compared to growth as determined by dry weight (

). (B) SDS-PAGE of culture filtrates from S. tendae NP51(pK11) and purified AFP1. Lanes 1 to 5, culture filtrate (40 µl) taken at time points (1 to 5) indicated by arrows in panel A; lane A, purified AFP1 (5 µg); lane M, molecular mass markers. Proteins were stained with Coomassie blue. AFP1 is marked by an arrow.

AFP1 was purified to apparent homogeneity by a two-step purification based on the stability and solubility of AFP1 at acidicpH; AFP1 has a calculated pI of 5.3. After precipitation of mostproteins from culture filtrates at pH 3.0, the remaining proteinswere separated by cation-exchange chromatography using S-Sepharoseequilibrated in 25 mM acetate buffer (pH 3.0). After elution ofcontaminating proteins with 0.2 M NaCl in 25 mM acetate buffer(pH 3.0), AFP1 was eluted with 0.3 M NaCl in the same buffer andappeared to be homogeneous on SDS-polyacrylamide gels (Fig. 4).Final recovery of AFP1 was 30%.

Properties of purified AFP1. The N-terminal amino acid sequence of AFP1 determined by Edman degradation revealed that 42 amino acid residues were cleavedfrom the N terminus of the afp1-encoded protein (Fig. 2). Themolecular mass of AFP1 was determined by electrospray mass spectrometryto be 9,862 ± 2.7 Da, which coincided with that deduced from thenucleotide sequence (9,860 Da). The molecular mass determinedby SDS-PAGE after AFP1 was reduced by dithiothreitol (Fig. 4)and gel filtration gave a considerably lower value of 6,100Da.

Native AFP1 did not react with Ellman's reagent, which detects free thiol groups, but gave a positive reaction after treatmentwith sodium borohydride, which indicated that Cys-6 and Cys-24of AFP1 form a disulfide bridge (Fig. 2). The reduced form ofAFP1 did not exhibit antifungal activity in agar diffusionassays.

AFP1 was stable over the pH range of 1.5 to 12 and resisted almost completely digestion by pepsin at pH 4 and 5 and by proteinaseK, pronase, or trypsin at pH 7 (data not shown). Heating purifiedAFP1 at temperatures between 70 and 100°C for 60 min reduced antifungalactivity to 50%.

Biological activity. The antimicrobial activity of AFP1 was determined by growth inhibition assay on agar plates seeded with various microorganisms(Table 1). AFP1 inhibited growth of specific ascomycetes; P.variotii was the most sensitive fungus tested. In contrast, AFP1had no effect on the growth of E. coli, Micrococcus luteus, S.lividans TK23, Mucor species, and yeasts. Growth of P. variotiiwas inhibited at AFP1 concentrations of >4 µg per well (Fig. 5).In addition, AFP1 applied to the growing front of a colony directlyinhibited hyphal growth of fungi that were affected in agar diffusionassays (shown for P. variotii in Fig. 5). Growth inhibition zonescaused by AFP1 were stable for weeks when test plates were furtherincubated at room temperature.

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TABLE 1. Biological activity of AFP1 in agar diffusion assays

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FIG. 5. Growth inhibition of P. variotii by purified AFP1. (A) Growth of spores in response to 4, 8, 10, 15, 20, and 30 µg of AFP1 per well (clockwise beginning at the top). (B) Growth of hyphae in response to 30 µg of AFP1 applied on the paper disk, placed at the growing front of a colony and incubated for further 48 h.

Combinations of AFP1 and the chitin synthetase inhibitor nikkomycin were tested against fungi affected by AFP1 to detect possiblesynergistic effects between the antifungal agents. Synergism wasclearly observed against Aspergillus species, especially A. fumigatus(Table 1).

Test for enzyme activities and polysaccharide binding. As the biological activity of AFP1 was exclusively directed against ascomycetes, AFP1 was assayed for enzyme activities directedagainst chitin and $beta$ -1,3-glucan, the main components of theircell wall (50). However, neither chitinase and $beta$ -1,3-glucanaseactivity nor the release of reducing sugars from cell walls ofP. variotii could be detected. Since AFP1 had limited sequencesimilarity to cellulose-binding domains, binding of fluorescein-labeledAFP1 to various polysaccharides and the cell wall of P. variotiiwas studied. Microscopy observations revealed that AFP1 bindsto crab shell chitin, chitosan, and P. variotii cell wall butdoes not to $beta$ -1,3-glucan (curdlan), crystalline cellulose (Avicel),and xylan (Fig. 6).

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FIG. 6. Binding of AFP1 to chitin, chitosan, and fungal cell walls. Fluorescein-labeled AFP1 was incubated overnight with crab shell chitin (A), crab shell chitosan (B), P. variotii cell wall (C), $beta$ -1,3-glucan (curdlan; D), Avicel (E), and xylan (F). After three washes with 100 mM Tris-HCl (pH 7.6)-150 mM NaCl, samples were analyzed by phase-contrast (left) and fluorescence (right) microscopy.

Effect of AFP1 on fungal morphology and its localization. The phenotypes of P. variotii and A. fumigatus affected by AFP1 were determined by inoculating 200 µl of complete medium (HA)containing various concentrations of AFP1 with conidia and cultivatingthe plates for 12 h. At 50 µg of AFP1 ml¹, approximately 80% of P. variotii conidia (4 to 6 µm) grew isotropicallyto large, round cells up to 25 µm in diameter. After washing andplating onto solid medium, the large germ spheres grew to formcolonies. The remaining conidia germinated normally and grew togerm spheres 11 µm in diameter and formed a germ tube (Fig. 7A).At higher concentrations of AFP1 (>75 µg ml¹), in addition to the large round cells, hyphal swelling was observed(data not shown). In contrast, large spheres were not observedfor A. fumigatus. At concentrations of 50 µg of AFP1 ml¹, A. fumigatus germinated and grew normally (Fig. 7D); at concentrationsof >75 µg of AFP1 ml¹, aberrant branching of hyphae and increased hyphal width wereobserved (Fig. 7C). Mycelia lysed easily upon mechanical force.

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FIG. 7. Effect of AFP1 on the morphology of P. variotii and A. fumigatus and its localization. P. variotii (A and B) and A. fumigatus (C and D) were grown in the presence of fluorescein-labeled AFP1 (A, B, and D, 50 µg ml¹; C, 75 µg ml¹) for 12 h and analyzed by phase-contrast (left) and fluorescence (right) microscopy. Scale bar represents 20 µm.

Fluorescein-labeled AFP1 (50 µg ml¹) was used to localize AFP1 on both fungi (Fig. 7). With P. variotii, most of the fluorescenceappeared on the surface of the large spheres, and fluorescencewas also detected along hyphae. With A. fumigatus, strong fluorescenceappeared at hyphal tips and at the wall of germinated conidiathat had formed a germtube.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The gene for the extracellular AFP1 from S. tendae Tü901 was cloned on a multicopy vector in a nikkomycin-nonproducing mutant.Overexpression was a prerequisite for detection of the gene bythe screening method used. Since AFP1 was produced in large amountsby the transformants and remained stable and soluble at acid pH,it was rapidly purified to homogeneity from culture filtrate.Mature AFP1 consists of 86 amino acid residues according to theN terminus defined by Edman degradation and the molecular massobtained by electrospray mass spectrometry. The estimation ofan apparent lower molecular mass for AFP1 by SDS-PAGE and gelfiltration might be due its relatively small size and an unusualmolecular shape caused by the presence of a disulfide bridge,which could influence the binding of SDS (5) and lead to deviationsfrom the ideal behavior in gel filtration. A significantly lowerapparent molecular mass has also been determined for the S. tendae4158 $alpha$ -amylase inhibitor tendamist, which consists of 74 aminoacids and contains two disulfide bridges (46).

The afp1 gene encodes a typical signal peptide required for secretion with three positively charged amino-terminal amino acidresidues (two Arg and one Lys) and a hydrophobic core region.However, extracellular AFP1 does not appear to be the direct productof cleavage by signal peptidase I, as the residues upstream ofthe determined N terminus of extracellular AFP1 (Gly-Pro-Thr)do not conform to the $-$ 1, $-$ 3 rule, which states that proline mustbe absent from positions $-$ 3 to +1 relative to the cleavage siteof signal peptidase I (48). Two sites that follow the $-$ 1, $-$ 3rule (Ala-Ala-Ala and Ala-Ser-Ala) and that are preceded by aturn-promoting proline at distances of 2 and 3 residues, respectively,are located 13 and 4 amino acid residues upstream of the N terminus.Since purified AFP1 from S. lividans(pK11) consisted of a smallproportion (10 to 20%) of the protein with five additional aminoacids (Ala-Ile-Gly-Pro-Thr-) at the N terminus (data not shown),AFP1 isolated from S. tendae NP51(pK11) might be the result ofextracellular processing subsequent to the initial signal peptidasecleavage. Similar phenomena have been reported for protein proteaseinhibitors from S. lividans and S. longisporus overproduced inS. lividans; the protein revealed amino-terminal amino acid heterogeneityin relation to the length of cultivation (44).

AFP1 is a chitin-binding protein that strongly interacted with crab shell chitin, chitosan, and fungal cell walls. Bindingof proteins to carbohydrates is mediated by aromatic residues,primarily tryptophan and tyrosine, through hydrogen-bonding andhydrophobic interactions (42). Three tryptophan residues ofbacterial cellulose-binding domains to which AFP1 shows sequencesimilarity have been shown to be exposed to one side of the domainand to be involved in protein-sugar binding (34, 52). AFP1has aromatic amino acid residues at the relevant positions: histidine,tyrosine, and tryptophan at positions 15, 36, and 40, respectively.Tryptophan, tyrosine, and histidine are also found at analogouspositions in cellulose-binding domains of distinct families ofproteins (45). Bacterial cellulose-binding domains are foundin many cellulases, xylanases, and other hemicellulases that havea modular structure (13). These enzymes appear to have evolvedfrom a limited number of ancestral sequences by domain fusionwith subsequent modifications of the domains. A significant transferof xylanase genes that fall into two distinct families seems tohave occurred between bacteria and eukaryotic microorganisms.Since the afp1 gene has features that are extraordinary for Streptomyces(a low G+C content of DNA and a poly[T] region and stem-loop structuredownstream of the gene), it is tempting to speculate that it mayhave evolved from a progenitor polysaccharide-binding domain ofmicroorganisms having a G+C content lower than that of Streptomyces.Many streptomycetes, including S. tendae Tü901, utilize chitinas sole carbon and nitrogen source and can be easily enrichedfrom soil on plates containing chitin as the only nutrient. WhetherAFP1 is part of the chitinolytic system that facilitates degradationof chitin in a way similar to that proposed for cellulose-bindingdomains in microbial plant cell wall hydrolases (26) is nowbeinginvestigated.

AFP1 represents the first chitin-binding protein from bacteria that exhibits antifungal activity. As antifungal activity hasalso been demonstrated for AFP1 isolated to homogeneity from E.coli BL21(DE3) cell extracts carrying the portion of the afp1gene for the mature AFP1 protein in the T7 RNA polymerase-basedpET11a (data not shown), there is no doubt that antifungal activityis caused by AFP1 alone. The chitin-binding proteins, CHB1 andCHB2, recently isolated from Streptomyces also bind to $alpha$ -chitinand fungal hyphae but have no antifungal activity (40). AFP1does not show sequence similarity to CHBs, which have a highermolecular mass (18.7 kDa) and an isoelectric point at alkalinepH (9.01). The antifungal property of AFP1 might be related toits small size, which would allow it to penetrate the fungal wall.An estimate of fungal wall pore size predicts that proteins largerthan 15 to 20 kDa will not be able to pass through the fungalwall (29). Chitin-binding proteins from plants that have antifungaleffects (e.g., Ac-AMPs from seeds of amaranth, nettle lectin,and hevein) are of small size (reference 35 and references herein).Members of the RP-4 family have molecular masses of 13 to 15 kDa(22). The most potent chitin-binding lectins are the 6-kDa Ac-AMPsthat act against a broad spectrum of fungal pathogens at concentrationsof 1 to 10 µg ml¹. The 8.5-kDa nettle lectin inhibits germ tube growth of sevenfungi at concentrations of 20 to 150 µg ml¹, which is the range required for antifungal activity of AFP1,while the 5-kDa hevein, which causes swelling of hyphae, is threeto five times lessactive.

The mechanism of growth inhibition by the plant chitin-binding proteins is not known. Microscopy studies revealed that fluorescein-labeledAFP1 preferentially binds to sites where cell wall synthesis takesplace: at conidia which grow isotropically by adding new wallmaterial uniformly in every direction and to hyphal tips (50).Therefore, it might be speculated that AFP1 interferes with cellwall synthesis by binding to nascent chitin, eventually cross-linkingthe polymer and interfering with growth polarity. The susceptibilityof chitin synthetase for the antibiotic nikkomycin appeared tobe enhanced in Aspergillus species, which are less sensitive tonikkomycin alone. Similar synergism has been reported for zeamatinand thaumatin-like proteins, which belong to the RP-5 family andfacilitate penetration of nikkomycin by interaction with the fungalmembrane (16, 36). In fungi, wall synthesis is coupled toexocytosis of vesicles containing wall-synthesizing enzymes andwall material, a process that determines growth polarity. Thetransport of vesicles is assumed to be mediated by a cytoskeleton,of which actin is the most important component. Actin is concentratedin areas of growth, and linkages between actin and plasmalemmahave been postulated (reference 15 and references therein).The factors that establish polarity and subsequent cell wall synthesisof filamentous fungi and that maintain polarity are relativelyunknown. Recently, eight Aspergillus nidulans mutants were isolatedand characterized. These mutants have defects in one of theseprocesses, and their germinated conidia and hyphae are misshapen(28).

The predominant effect of AFP1 on P. variotii occurred during spore germination. AFP1 interfered with polarized growth andprevented the emergence of a normal germ tube but allowed nonpolargrowth, leading to large spherical cells with a rigid wall. Inaddition, AFP1 interfered with polarized growth at hyphal tips,leading to abnormal branching and swollen hyphae with weakenedwalls that did not resist internal turgor pressure upon mechanicalstress. The different effects of AFP1 on P. variotii and A. fumigatus,where AFP1 appeared only to interfere with growth polarity ofhyphae and the selectivity of AFP1 toward ascomycetes, may bedue to the cell wall-associated proteins, which might act as aphysical barrier for AFP1 and determine accessibility of the target.Cell wall proteins have been shown to be determinants of resistanceof Saccharomyces cerevisiae toward tobacco osmotin and are presumedto mask binding sites in the plasma membrane that mediate osmotinaction (55). AFP1 may be a valuable tool for studying chitinsynthesis in filamentous fungi and its coupling to processes involvedin determination of growth polarity and for investigating determinantsofresistance.

	ACKNOWLEDGMENTS

We thank S. Stevanovic and J. Metzger (Institute of Organic Chemistry, University of Tübingen) for analytical support, B.Lattermann (Max-Planck-Institut für Entwicklungsbiologie, Tübingen,Germany) for introduction to photomicroscopy, P. L. Huynh andG. Scheer for making photographs, and K. A. Brune for editingthemanuscript.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 323, A4, andC2).

	FOOTNOTES

^* Corresponding author. Mailing address: Mikrobiologie/Biotechnologie, Universität Tübingen, Auf der Morgenstelle 15, D-72076Tübingen, Germany. Phone: (49) 7071 297 7620. Fax: (49) 707129 4634. E-mail: christiane.bormann{at}uni-tuebingen.de.

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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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1.	Abad, L. R., M. P. D'Urzo, D. Liu, M. L. Narasimhan, M. Reuveni, J. K. Zhu, X. Niu, S. N. K., P. M. Hasegawa, and R. A. Bressan. 1996. Antifungal activity of tobacco osmotin has specificity and involves plasma membrane permeabilization. Plant Sci. 118:11-23.
2.	Altschul, S. F., T. L. Madden, A. A. Schäffer, J. Zhang, Z. Zhang, W. Miller, and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].
3.	Bormann, C., K. Aberle, H.-P. Fiedler, and H. Schrempf. 1990. Genetic complementation of Streptomyces tendae deficient in nikkomycin production. Appl. Microbiol. Biotechnol. 32:424-430[Medline].
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