Identification and Characterization of a Gene Cluster for Synthesis of the Polyketide Antibiotic 2,4-Diacetylphloroglucinol from Pseudomonas fluorescens Q2-87

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Journal of Bacteriology, May 1999, p. 3155-3163, Vol. 181, No. 10
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Identification and Characterization of a Gene Cluster for Synthesis of the Polyketide Antibiotic 2,4-Diacetylphloroglucinol from Pseudomonas fluorescens Q2-87

M. Gita Bangera¹^, and Linda S. Thomashow¹^,²^,^*

Department of Microbiology, Washington State University, Pullman, Washington 99164-4233,¹ and USDA Agricultural Research Service, Root Disease and Biological Control Research Unit, Washington State University, Pullman, Washington 99164-6430²

Received 4 March 1999/Accepted 12 March 1999

	ABSTRACT

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The polyketide metabolite 2,4-diacetylphloroglucinol (2,4-DAPG) is produced by many strains of fluorescent Pseudomonas spp.with biocontrol activity against soilborne fungal plant pathogens.Genes required for 2,4-DAPG synthesis by P. fluorescens Q2-87are encoded by a 6.5-kb fragment of genomic DNA that can transferproduction of 2,4-DAPG to 2,4-DAPG-nonproducing recipient Pseudomonasstrains. In this study the nucleotide sequence was determinedfor the 6.5-kb fragment and flanking regions of genomic DNA fromstrain Q2-87. Six open reading frames were identified, four ofwhich (phlACBD) comprise an operon that includes a set of threegenes (phlACB) conserved between eubacteria and archaebacteriaand a gene (phlD) encoding a polyketide synthase with homologyto chalcone and stilbene synthases from plants. The biosyntheticoperon is flanked on either side by phlE and phlF, which coderespectively for putative efflux and regulatory (repressor) proteins.Expression in Escherichia coli of phlA, phlC, phlB, and phlD,individually or in combination, identified a novel polyketidebiosynthetic pathway in which PhlD is responsible for the productionof monoacetylphloroglucinol (MAPG). PhlA, PhlC, and PhlB are necessaryto convert MAPG to 2,4-DAPG, and they also may function in thesynthesis ofMAPG.

	INTRODUCTION

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Phloroglucinols are phenolic bacterial and plant metabolites with broad-spectrum antiviral, antibacterial, antifungal, antihelminthic,and phytotoxic properties. The compound 2,4-diacetylphloroglucinol(2,4-DAPG), which is produced by certain plant-associated fluorescentPseudomonas species of worldwide origin (23, 57), is of particularsignificance to agriculture because of its activity in situ againsta variety of root and seedling pathogens of plants (reviewed inreference 57). 2,4-DAPG production is the major determinantin the ability of P. fluorescens Q2-87 to suppress Gaeumannomycesgraminis var. tritici, the fungal pathogen that causes take-alldisease of wheat. The 2,4-DAPG-nonproducing Tn5 mutant Q2-87::Tn5-1was unable to inhibit the pathogen in vitro and did not protectwheat against take-all (16, 61). Interest in 2,4-DAPG-producingpseudomonads has focused not only on their potential as introducedagents for biological control but also on their activity in naturalagroecosystems. Indigenous populations of 2,4-DAPG-producing Pseudomonasspp. have a key role in the suppressiveness to take-all (take-alldecline) that develops in some soils during extended monocultureof wheat in the presence of the take-all pathogen (43-45).

2,4-DAPG is thought to be derived from monoacetylphloroglucinol (MAPG), and an acetyltransferase activity capable of convertingMAPG to 2,4-DAPG has been described in Pseudomonas sp. strainF113 (52). No precursors of MAPG have yet been identified, butthe hydroxyl groups at alternating positions on the phloroglucinolring are consistent with biosynthesis via a polyketide mechanism.Naturally occurring polyketides are produced by the successivecondensation of small carboxylic acids in a process that resemblesfatty acid synthesis. The genes encoding polyketide synthases(PKSs) show similarities to one other as well as to genes forfatty acid synthases (18, 20). Three types of PKS are known.Type I enzymes are large multifunctional proteins with domainsthat catalyze the individual steps of the pathway in a nonreiterativemanner. In contrast, type II PKSs are complexes of four to sixmono- or bifunctional proteins that can function reiterativelyto assemble the polyketide molecule (20). A third kind of PKS,which we designate type III, is exemplified by members of thechalcone synthase (CHS) and stilbene synthase (STS) family fromplants. These enzymes consist of a homodimeric protein that issufficient to perform the condensation and cyclization steps neededto produce their phenolic products (30, 48). Type I and typeII PKS enzyme systems have been studied extensively in Streptomycesspp. and other actinomycetes, and recent evidence indicates thatboth kinds of synthases also function in Pseudomonas spp. Genescharacteristic of a type I PKS have been identified in DNA requiredfor the production of the antifungal metabolite pyoluteorin byPseudomonas fluorescens Pf-5 (35), and a type II PKS is involvedin the synthesis of coronafacic acid (CFA), the polyketide componentof the phytotoxin coronatine produced by Pseudomonas syringae(27, 40). A type I-like PKS coding region also has been identifiedadjacent to the CFA biosynthetic cluster, suggesting that CFAsynthesis may involve a unique combination of mono- and multifunctionalenzymes (46).

Genes sufficient to confer the ability to produce 2,4-DAPG on 2,4-DAPG-nonproducing recipient strains of Pseudomonas spp.were localized to a 6.5-kb DNA fragment from P. fluorescens Q2-87in a previous study. Analysis of this fragment by transposon mutagenesiswith Tn3HoHo1 identified a region spanning approximately 5 kbthat contained at least two divergently oriented transcriptionalunits required for DAPG production (3). The goal of the presentstudy was to elucidate the role of these genes in the synthesisof 2,4-DAPG and its precursor, MAPG. Nucleotide sequence analysisof the region revealed six genes organized in three transcriptionalunits. Four genes comprise the operon phlACBD, and expressionstudies indicated that the protein products of all four are requiredfor the synthesis of both MAPG and 2,4-DAPG. The products of phlACBDresemble neither type I nor type II PKS enzyme systems. Rather,PhlD exhibits striking homology to plant chalcone synthases, indicatingthat phloroglucinol synthesis is mediated by a novel kind of PKSnot previously described in microorganisms. The biosynthetic operonis flanked on either side by the separately transcribed genesphlE and phlF, which code respectively for putative efflux andregulatory (repressor) proteins that are not absolutely requiredfor phloroglucinolproduction.

	MATERIALS AND METHODS

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Organisms and culture conditions. Plasmids and bacterial strains used in this study are described in Table 1. Cultures of fluorescent Pseudomonas strains weregrown at 28°C in yeast malt broth (3) for 2,4-DAPG extractionand in Luria Bertani (LB) medium (47) for other manipulations.Escherichia coli DH5 $alpha$ and BL21(DE3) were used as hosts for plasmidconstruction and protein expression studies, respectively. E.coli cultures were grown in LB medium for routine purposes, intryptone phosphate broth (32) for protein expression, in M9minimal medium for ³⁵S labeling, or in M9 medium with 0.02% yeast extract for 2,4-DAPGextraction. Ampicillin was included at 100 µg/ml for routine workwith plasmid-containing E. coli strains and at 400 µg/ml duringprotein expression. Kanamycin and tetracycline were used at 50and 25 µg/ml, respectively.

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TABLE 1. Plasmids and strains used in this study

DNA manipulations. Plasmid DNA was isolated by the method of Birnboim and Doly (5). Restriction and ligation reactions and agarose gel electrophoresiswere performed by standard methods (47) or as directed by thesuppliers. DNA fragments were recovered from agarose gels by thefreeze-squeeze method (56). Competent cells were prepared fortransformation according to the method of Morrison (33).

Sequence analysis. Subclones from pMON5122 and pMON5120 (Table 1) were generated by using convenient restriction sites and inserted into thecloning vector pIC19H. DNA sequences were determined at the NucleicAcid Research Facility at Iowa State University, Ames, with anABI automated sequencer. Oligonucleotides complementary to internalsequences were used as primers to complete the sequencing of largerfragments.

Sequence data were analyzed with the University of Wisconsin Genetics Computer Group package, version 8.0 (13). DNA sequenceswere compiled with GELASSEMBLE, and open reading frames (ORFs)were identified and codon usage was analyzed with MAP and FRAMES.The GenBank and EMBL databases were searched for sequence similaritiesby using the programs FASTA, BLAST, and MOTIFs. The PROSITE databasewas searched for protein domain similarities by using the ExPASymolecular biology server (1). Multiple sequences were alignedwith PILEUP and PRETTYBOX (13). Kyte-Doolittle hydropathy plotswere generated with PK23, a program developed by the VADMS centerat Washington State University, Pullman. The significance of thesimilarity of a predicted protein to known proteins was determinedby calculating the binary comparison score (Z score). Pairwisealignments were obtained by using the program GAP (gap weight= 3), and the resulting percent identities, percent similarities,alignment scores (A), mean random alignment scores (R), and standarddeviations (SD) (n = 100) were noted. Z scores were then calculatedby the equation (A $-$ R)/SD.

RNA isolation and Northern analysis. Total RNA was isolated with the RNeasy kit (Qiagen, Chatsworth, Calif.) from 400- or 500-µl samples of 4-ml cultures of P.fluorescens grown at 28°C with vigorous shaking. The followingchanges were made to the RNeasy protocol: the membrane was incubatedat room temperature for 5 min after the addition of wash bufferRW1 and again after the addition of RNase-free water before centrifugation.RNA samples separated on agarose gels were transferred to BrightStar-Pluspositively charged nylon membranes (Ambion, Austin, Tex.) with7.5 mM sodium hydroxide as the transfer buffer. Probes were labeledand detected with the BrightStar nonradioactive labeling and detectionsystem(Ambion).

Plasmid constructions. Nine plasmids were constructed for gene function analysis. Introduction of the 6.5-kb fragment from pMON5122 into pT7-5 gavepPHL5140. Plasmid pPHL5141 was created by cloning the 4.1-kb SalI-EcoRIfragment of pPHL5140 into pT7-5. Plasmid pPHL5141A was generated by deleting the EagI-EcoRI fragment from the rightend of the insert in pPHL5141. pPHL5141 was digested with SphI,the ends were filled in with the Klenow fragment of E. coli DNApolymerase, and the plasmid was religated to form pPHL5141B. pPHL5141C was produced by digestion of pPHL5141 with EcoRV and religationto eliminate a 0.7-kb fragment. Finally, a parallel set of threeplasmids in which the 3' end of the 7.2-kb fragment was reintroducedinto the pPHL5141 derivatives was generated by a two-step cloningstrategy. The SalI-StuI fragment from pPHL5140 was cloned in pIC19Hto give pSS1. This fragment was then isolated as a SalI-HindIIIfragment and ligated into SalI-HindIII-digested pPHL5141A, pPHL5141B, and pPHl5142C to give pPHL5142A, pPHL5142B, and pPHl5142C, respectively (Table 1; Fig. 1).

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FIG. 1. Genes identified in the 2,4-DAPG biosynthetic locus are indicated by black horizontal arrows. The vertical arrow indicates the site of Tn5 insertion in Q2-87::Tn5-1. Key plasmids used in assigning functions to the phl genes are shown. Construction of these plasmids is described in Materials and Methods. Restriction sites: A, AccI, B, BamHI; E, EcoRV; Eg, EagI; P, PstI; R, EcoRI; S, SalI; Sp, SphI; St, StuI.

SDS-PAGE and protein labeling. Proteins expressed in E. coli from the nine plasmids described above were analyzed by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) both with and without [³⁵S]methionine labeling in vivo. For nonradioactive protein analysis,overnight cultures were diluted 50-fold and grown with shakingto an A₆₀₀ of 0.6. Cells from 1 ml of culture were harvested andsuspended in 25 to 40 µl of 1× Laemmli buffer, and a 5-µl samplewas analyzed by electrophoresis on 10 or 12% acrylamide gels (47).Proteins were radiolabeled in vivo as described by Ausubel etal. (2), except that transcription from the T7 promoter wasinduced with 3 mM isopropyl- $beta$ -D-thiogalactoside (IPTG) for 30min. Incubation was continued for 20 min at 42°C with rifampin(200 µg/ml), and then 10 µCi of [³⁵S]methionine was added and incubation was continued for 5 min.Gels were stained with Coomassie brilliant blue R250 in methanol-aceticacid-water (4.5:4.5:1) for nonradioactive samples or with Coomassiebrilliant blue R250 in boiling 7% acetic acid beforeautoradiography.

N-terminal sequencing of PhlA. Proteins from E. coli BL21(DE3)(pPHL5141) were separated on an SDS-12% polyacrylamide gel and transferred to a polyvinylidenedifluoride membrane (Millipore Corporation, Bedford, Mass.) witha Mini Trans-Blot apparatus (Bio-Rad Laboratories, Hercules, Calif.).The membrane was stained with Coomassie brilliant blue R250 inmethanol-acetic acid-water (4.5:4.5:1) and destained in the samesolvent. After washing the membrane six times with reagent-gradewater, the PhlA band was excised and the protein sequence wasdetermined directly from the immobilized band at the Laboratoryfor Bioanalysis and Biotechnology at Washington State Universitywith an Applied Biosystems 475A proteinsequencer.

Extraction and detection of metabolites. MAPG and 2,4-DAPG were extracted from 4-day-old cultures of E. coli or Pseudomonas as described previously (3). Expressionof the locus in E. coli BL21(DE3) was based on the leaky lac repressorcontrol of expression from the T7 promoter since expression inthese cultures was not induced with IPTG. For analysis of theconversion of MAPG to 2,4-DAPG, MAPG was added to a concentrationof 10 µg/ml to 24-h-old cultures and the cultures were incubatedfor 3 additional days. Metabolites were extracted as describedabove and analyzed by high-pressure liquid chromatography accordingto the method of Bonsall et al. (6).

Nucleotide sequence accession number. The nucleotide sequence of the 7,198-bp DNA region described here is available in the EMBL, GenBank, and DDBJ data librariesunder the accession no. U41818.

	RESULTS

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Nucleotide sequence analysis. The nucleotide sequence of 7,198 bp of DNA including the 6.5-kb fragment from pMON5122 and about 500 bases adjacent to itfrom pMON5120 was determined. Six ORFs were identified with codonusage conforming to that established for Pseudomonas spp. TheseORFs were designated phlA, phlC, phlB, phlD, phlE, and phlF. ORFsphlA, phlC, phlB, phlD, and phlE have a common transcriptionalorientation, and phlF is oppositely oriented (Fig. 1), as predictedearlier by transcriptional analysis with Tn3HoHo1 (3). A putativeATG start codon (in boldface type) for phlA (CATTCTGGAAATG)is not preceded by a consensus ribosome binding site, but a GTGcodon (in boldface type) with such a site (underlined) (GGAGGAAGTACACGTG)was identified 288 bases upstream of the ATG. Each of the otherORFs has an appropriately positioned potential ribosome bindingsite, except for phlE, which is preceded by a sequence rich inA and G residues (AAAGAAGGGGAAGAACATG). The characteristicsof the predicted ORF products are described in Table 2.

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TABLE 2. ORFs in the 2, 4-DAPG biosynthetic cluster

The putative product of phlA shows 26% identity and 48% similarity to the 33-kDa fabH gene product $beta$ -ketoacyl-acyl carrierprotein synthase III (KAS III) from E. coli (59). Similarityto KAS III enzymes from other organisms was very poor (data notshown). Further inspection revealed that PhlA lacks the activesite cysteine residue (C112 of FabH). An imperfect phosphopantetheine-bindingmotif (IGADTINRNTAPGDL) was identified at residue 143 in whicha threonine (underlined) replaces the conserved pantotheine-bindingserine residue. The ORF designated phlC initiates with an ATGcodon 32 bp downstream of the phlA stop codon. The predicted phlCproduct shows 28% identity and 50% similarity to the N-terminalthiolase domain of rat sterol carrier protein x (SCPx). PhlC carriesan acetyl-coenzyme A (CoA) binding site containing the activecysteine residue as well as a glycine-rich C-terminal region conserved(36, 53) among thiolases (Fig. 2) and ketoacyl-condensingenzymes (data not shown). The ATG start codon for phlB is 11 basesdownstream of phlC. No structural motifs suggestive of a functionfor phlB were identified. However, the predicted proteins PhlA,PhlC, and PhlB have homology with the predicted products of theaca operon from the archaebacterium Pyrococcus furiosus and withthe predicted proteins MJ1545, MJ1549, and MJ1552 from Methanococcusjannaschii (7, 25). ORF phlD is separated from phlB by 155bases and shows homology at the predicted protein sequence levelto CHS/STS genes from higher plants (31% identity, 53% similarity)(Table 2). Both the active site region (for CHS, QQGC¹⁶⁹FAG; for PhlD, QLGC¹³⁸VAG) including the catalytic cysteine (underlined) (26) anda highly conserved family signature sequence (for CHS, ³⁷⁴VGVLFGFGPGLTVE; for PhlD, ³²⁸TGMLAAFGPGFTAE) common to CHS/STS enzymes (12) were found inPhlD. PhlD also shows similarity to three bacterial CHS homologuesof unknown function (60) (GenBank accession no. L77246 andZ85982).

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FIG. 2. Important residues conserved in PhlC. (A) Alignment of cysteine 88 (*) of PhlC with the catalytic active site cysteine of thiolases. (B) Alignment of histidine 349 ( $black-down-triangle$ ) and neighboring glycine residues of PhlC. Cysteine 378 (

), a key active site residue in type II thiolases, is absent from PhlC, SCPx, and AcaB. In both panels, the compared proteins are chrom_aat, Chromatium vinosum acetoacetyl-CoA thiolase (accession. no. L01112); alcal_aat, Alcaligenes eutrophus acetoacetyl-CoA thiolase (accession no. J04987); ratmit_aat, rat mitochondrial acetoacetyl-CoA thiolase (accession no. D13921); ratmit_thiol, rat mitochondrial oxoacyl-CoA thiolase (accession no. X05341); rat_pota, rat peroxisomal oxoacyl-CoA thiolase A (accession no. M32801); rat_potb, rat peroxisomal oxoacyl-CoA thiolase B (accession no. J02749); ecfada, E. coli 3-ketoacyl-CoA thiolase (accession no. P21151); caen_aat, Caenorhabditis elegans acetyl-CoA acetyltransferase (accession no. M77697); scpx, mouse sterol carrier protein 2 precursor (accession no. P32020); and acab, P. furiosus acetyl-CoA synthase. Numbers to the right of the alignment are amino acid residue numbers.

A palindromic DNA sequence (¹⁷⁶²CCAGGGGCGGATCCGCCCCCGG) lies between phlD and phlE. PhlE is homologous (24% identity and 50% similarity)with Staphylococcus aureus NorA protein (63), a multidrug effluxtransporter that belongs to the transmembrane solute facilitatorsuperfamily of membrane permeases. PhlE retains conserved structuralfeatures of these integral membrane permeases, including a centralhydrophilic loop bordered on either side by six hydrophobic $alpha$ -helices(Fig. 3).

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FIG. 3. Kyte-Doolittle hydropathy plots of PhlE and S. aureus NorA protein. Both plots show central hydrophilic loops flanked by twelve hydrophobic, potential membrane spanning regions (window size = 19).

The phlF start codon was located 416 bp upstream of the start codon for phlA. The intervening region contains no ORFs, isAT-rich, and presumably contains the phlA and phlF promoters.PhlF is homologous (25% identity and 48% similarity) with a putativerepressor gene in the rapamycin biosynthetic locus of Streptomyceshygroscopicus (50). Similarity with other repressor proteins,such as tetR, is concentrated within a helix-turn-helix domain(residues 34 to 64) typical of known DNA-binding regulatory proteins,as shown below. The top sequence is a consensus of helix-turn-helixdomains, and X represents any amino acid (1).

Consensus GYX₃SIX₂VX₅VSXPXIYXHFXNKX₂L
PhlF 34 GYX₃SIX₂VX₅ASXPXIYXWWXNKX₂L64

Northern analysis. The small intergenic distances between phlA, phlC, and phlB indicated that they might form an operon. However, it was notclear whether phlD was included in this operon or was transcribedseparately. To address this question, total RNA was isolated from3- and 24-h-old cultures of Q2-87. RNA from 3-h-old cultures ofQ69c-80, a 2,4-DAPG-nonproducing Pseudomonas strain, was usedas a negative control. A fourth sample contained RNA from a 24-h-oldculture of Q69c-80::miniTn5Phl, which includes sequences frompMON5122 on a chromosomally located mini-Tn5 transposon (24).Following electrophoresis and transfer, the RNA was hybridizedeither with an EcoRV fragment encompassing the central portionof phlC or with an AccI-BamHI fragment containing the entire phlDregion (Fig. 4). No RNA was detected in Q69c-80 by either probe.Both probes detected RNAs of similar sizes in the 24-h Q2-87 culture;the phlC probe, which was of higher specific activity than thephlD probe, also detected this RNA in the 3-h-old culture of Q2-87(Fig. 4). Both probes identified a slightly smaller transcriptin RNA from Q69c-80::miniTn5Phl.

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FIG. 4. Northern blot analysis of phl mRNA. Total RNA was isolated at 3 h (lanes 1 and 3) and 24 h (lanes 2 and 4) from P. fluorescens Q69c-80 (lanes 1), P. fluorescens Q69c-80::miniTn5Phl (lanes 2), and P. fluorescens Q2-87 (lanes 3 and 4). The probes used were a 0.7-kb EcoRV fragment specific for phlC (A) and a 1.1-kb AccI-BamHI fragment containing the entire phlD region (B). Positions of the 23S and 16S RNAs are shown. *, transcript detected from wild-type Q2-87 strains; **, smaller transcript detected in Q69c-80::miniTn5Phl.

Gene function analysis. Both MAPG and 2,4-DAPG were identified by HPLC in extracts from P. fluorescens Q2-87. Strain Q2-87::Tn5-1, which containsa transposon in phlD, produced no detectable MAPG or 2,4-DAPG.However, 2,4-DAPG was produced when the strain was provided withexogenous MAPG (Table 3), suggesting that PhlD is necessary forsynthesis of MAPG and that PhlA, PhlC, and PhlB are sufficientto perform the conversion of MAPG to 2,4-DAPG. To further dissectthe roles played by the different ORFs, nine plasmids were constructedin which the putative 2,4-DAPG biosynthetic genes were placedunder the transcriptional control of the strong, IPTG-induciblephage T7 promoter in plasmid pT7-5. SDS-PAGE analysis helped toidentify the proteins expressed by E. coli BL21(DE3) carryingthese plasmids and to detect the loss of the appropriate proteinon introduction of a mutation (Fig. 5).

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TABLE 3. Functional analysis of phl genes

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FIG. 5. Autoradiograph of polypeptides labeled with [³⁵S]methionine and resolved by electrophoresis in SDS-polyacrylamide gels. Samples were prepared from E. coli BL21(DE3) containing the indicated plasmids. The DNA fragments inserted in pT7-5 for gene expression are illustrated in Fig. 1. Top panel, 10% acrylamide gel; bottom panel, 12% acrylamide gel. Positions of phl gene products are indicated on the right; D* indicates the truncated PhlD product produced by strains expressing pPHL5141 and its derivatives. Positions of molecular size markers are given on the left in kilodaltons. Lanes: 1, pT7-5; 2, pPHL5140; 3, pPHL5141; 4, pPHL5142A; 5, pPHL5142B; 6, pPHL5142C.

Plasmid pPHL5140 enabled the production of both MAPG and 2,4-DAPG. To confirm that PhlA, PhlC, and PhlB were sufficient toconvert MAPG to 2,4-DAPG, pPHL5141, which contains phlA, phlC,phlB, and a truncated phlD gene encoding only the first 126 aminoacid residues of PhlD, was generated. Neither MAPG nor 2,4-DAPGwas detected in extracts from E. coli BL21(DE3)(pPHL5141), butMAPG added to 24-h-old cultures was converted to 2,4-DAPG. Mutationswere then introduced into phlA, phlC, and phlB in pPHL5141 todetermine which of them was required to carry out the conversion.pPHL5141A lacks the ribosome binding site and the first 90 N-terminal aminoacids of phlA, pPHL5141B has a frameshift mutation in phlB, and pPHL5141C carries a deletion in phlC. These mutations did not prevent theexpression of downstream genes (Fig. 5). E. coli containing pPHL5141A, pPHL5141B, or pPHL5141C failed to convert MAPG to 2,4-DAPG.

Finally, to clarify whether phlD was sufficient for the synthesis of MAPG or if phlA, phlC, or phlB also was required, phlDwas reconstructed in pPHL5141A, pPHL5141B, and pPHL5141C to obtain pPHL5142A, pPHL5142B, and pPHL5142C. These plasmids each contain a functional phlD gene but are defectivein phlA, phlB, or phlC, respectively. Cultures of E. coli BL21(DE3)expressing these plasmids produced neither MAPG nor 2,4-DAPG (Table3), although in LB medium they exhibited a reddish color similarto that observed in uninoculated LB medium supplemented withMAPG.

Protein expression in E. coli and N-terminal sequencing of PhlA. E. coli BL21(DE3)(pPHL5140) produced four unique proteins with relative molecular masses corresponding to those predictedfor PhlA, PhlB, PhlC, and PhlD. Due to the high level of expressionfrom the T7 promoter, all four proteins were visible on stainedacrylamide gels even without radiolabeling. The same unique proteinswere present in samples labeled with [³⁵S]methionine (Fig. 5). No unique band corresponding in size toPhlE was detected by either method. PhlA and PhlD are very similarin predicted size (37.9 and 38.4 kDa, respectively) but were successfullyresolved after electrophoresis in an SDS-10% polyacrylamide gel.Mutations in individual ORFs resulted in the disappearance ofthe corresponding protein band from the gel. PhlC was the mostpoorly expressed of all the proteins, while PhlB and PhlD wereexpressed more strongly. Strains expressing the PhlD plasmid pPHL5141 and its derivatives produced the truncated proteinPhlD*.

To identify which of the two potential start sites detected by sequence analysis of phlA was functional, the N-terminal sequenceof PhlA expressed from pPHL5141 in E. coli was determined. Thefirst eight amino acids detected, MNKVGIVS, corresponded to thepredicted sequence from the GTG startsite.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Six genes, designated phlA, phlC, phlB, phlD, phlE, and phlF, were identified in a 7.2-kb DNA fragment from P. fluorescensQ2-87. Each of these exhibited significant homology (Z scores> 9) with other known genes, indicating common evolutionary originsand suggesting mechanisms for the regulation, synthesis, and exportofDAPG.

PhlD is essential for MAPG synthesis (Fig. 6). In both P. fluorescens Q2-87 and in E. coli expressing phl genes, MAPG wassynthesized only in the presence of PhlD; in its absence, thecells converted exogenous MAPG to 2,4-DAPG but were unable toproduce either compound themselves. The homology between PhlDand CHS/STS enzymes from plants is surprising, as until now allthe microbial polyketide antibiotics have been found to be synthesizedvia type I or type II PKSs (10, 20, 22, 31, 35, 46).The structural similarities between PhlD and members of the CHS/STSfamily point to a common evolutionary origin, and the functionalparallels in the roles they play in plant defense provoke speculationas to possible instances of gene exchange between plants and theirbacterial colonists (4, 9).

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FIG. 6. Proposed roles of PhlA, PhlB, PhlC, and PhlD in the biosynthesis of MAPG and 2,4-DAPG. Enz, enzyme.

Unlike the multidomain (type I) and multiprotein (type II) PKSs, CHS/STS enzymes consist simply of a homodimer of 42-kDa subunitssufficient to catalyze the three condensation reactions, the cyclizationreaction, and, for the STSs, the decarboxylation reaction requiredto generate their particular products (58; reviewed in references30 and 48). The recruitment of such a unique enzyme for 2,4-DAPGproduction by strain Q2-87 suggests that other features characteristicof the CHS/STS biosynthetic mechanism might be present as well.For example, these enzymes differ from type I and type II PKSsin lacking an acyl carrier protein component; instead, they utilizeCoA esters of carboxylic acids as a source of extender units.This preference may explain the absence from the phl operon ofan acyl carrier protein gene comparable to those found in typeII PKSs. Further, CHS/STS enzymes (as far as is known) acceptonly malonyl-CoA as extender units, unlike type I enzyme complexes,which can incorporate branched acyl moieties. This would mandatethat 2,4-DAPG be synthesized via MAPG rather than directly bycondensation of other acyl-CoA substrates. Finally, although thenatural substrate of CHS/STS enzymes is 4-coumaroyl-CoA, theyexhibit broad substrate specificity in vitro, producing acylphloroglucinolcompounds from butyryl-CoA and hexanoyl-CoA primer molecules (19,49). By analogy, we postulate that PhlD catalyzes the condensationof a linear primer molecule, probably acetoacetyl-CoA.

That the products of phlA, phlC, and phlB function collectively is supported both by the fact that mutations in any one ofthe three genes give rise to a common phenotype and by conservationof a similar gene cluster in the archaebacterium P. furiosus (25).PhlA, PhlC and PhlB appear to have a dual role in 2,4-DAPG synthesis(Fig. 6). First, all three are necessary and sufficient for theconversion of MAPG to 2,4-DAPG. This acetylation reaction correspondsto an MAPG acetyltransferase activity described previously incell extracts of Pseudomonas sp. strain F113 (52). Second, theyalso appear to be required for the synthesis of MAPG, perhapsby catalyzing a condensation reaction needed to provide the primerunit forPhlD.

Sequence analysis gives only limited insight into the functions of PhlA and PhlB. PhlB lacks both recognizable motifs andsimilarity with other known proteins, and although PhlA is homologouswith FabH from E. coli, it contains an imperfect phosphopantetheine-bindingmotif with a threonine residue in place of the serine throughwhich the prosthetic group invariably is esterified. This motifis unlikely to be functional, as a similar substitution in a spinachacyl carrier protein I did not bind the phosphopantetheine group(21). PhlA also lacks the essential cysteine present in theactive site region of condensing enzymes. It is significant thatsuch cysteine-deficient ketosynthase homologues are integral tothe basic architecture of bacterial type II PKSs, where they helpto determine the chain length of the poly- $beta$ -ketone intermediateprior to cyclization (20). Whether PhlA functions as a chainlength factor, perhaps through interactions with PhlD, remainsto bedetermined.

Only PhlC contains structural features typical of condensing enzymes, and these features are consistent with roles in bothprimer unit synthesis and MAPG acetylation. For example, cysteine-88of PhlC aligns with the catalytic cysteine in the active siteof thiolases (Fig. 2A) and condensing enzymes and is the likelybinding site for acetyl-CoA prior to the reaction leading to synthesisof acetoacetyl-CoA, the putative MAPG primer unit. A second conservedregion includes the sequence ³⁴⁶GHASGCDG (Fig. 2B). It is noteworthy that this histidine residueis the only one conserved among condensing enzymes and thiolases(53). We speculate that in PhlC, it may form part of the bindingsite for a malonyl thioester, the extender unit in biosyntheticcondensation reactions except those catalyzed by type II thiolasesthat use acetyl-CoA to generate acetoacetyl-CoA. Although we predictthat PhlC generates acetoacetyl-CoA, as do type II thiolases,PhlC differs from the latter in lacking an equivalent to cysteine378, a key active site residue (37) (Fig. 2B), and it thereforeis unlikely that PhlC uses acetyl-CoA as an extender unit. Itis curious that PhlC most closely resembles the thiolase domainof SCPx, the product of an apparent fusion of genes for thiolaseand a small mammalian protein important in the intracellular transportof lipids and sterols, particularly cholesterol (36, 41, 51).Similarity between the SCPx thiolase domain and PhlC extends overthe entire length of the two sequences, rather than only in thekey catalytic regions, suggesting that the two proteins may havecommon conformational features that could facilitate an interactionbetween PhlC and MAPG in a manner analogous to that between SCPxand its sterolligands.

PhlE retains structural features of integral membrane permeases including the archetypal tetracycline-H⁺ antiporters (34, 38, 39) and transport proteins associatedwith resistance and encoded within the biosynthetic clusters forpolyketide antibiotics (11, 14). That PhlE functions in theexport of 2,4-DAPG and/or MAPG is supported by an earlier observation(3) that certain Tn3HoHo1 insertions in phlE were correlatedwith reduced 2,4-DAPG production and loss of the red pigment characteristicof phloroglucinol compounds. These insertions were interspersedwith others that had no effect on pigmentation, suggesting thatPhlE has multiple functional domains which may correspond to thehydrophilic and transmembrane segments predicted by sequence analysis.No protein corresponding to PhlE was detected in E. coli expressingphlACBD under the control of a T7 promoter, indicating that thetwo are likely to be separately transcribed and that a 22-basepalindrome located between phlD and phlE functions as a transcriptionalterminator.

The product of the divergently transcribed phlF gene at the 5' end of the 2,4-DAPG biosynthetic operon contains a helix-turn-helixmotif strongly predictive of DNA-binding activity and similarto that of well-characterized repressor genes, including membersof the TetR family. Two additional observations further supportthe hypothesis that PhlF is a negative regulator of 2,4-DAPG biosynthesis.First, whereas pMON5122 (which lacks the 73 codons at the 3' endof phlF) transferred 2,4-DAPG biosynthetic capability to previouslynonproducing strains of Pseudomonas, larger cloned segments containingflanking sequences that included the intact phlF gene did not.This previously led us to postulate that negative regulatory elementsmight reside upstream of the 2,4-DAPG locus (3). Secondly,derivatives of P. fluorescens Q69c-80 containing a single chromosomalcopy of phlACBDE and the 3'-truncated phlF gene from pMON5122produced up to several hundred-fold more 2,4-DAPG than did wild-typeQ2-87 (24). Similar truncation of Tn10 and class E tetR tetracyclinerepressor proteins derepresses expression of the tetracyclineresistance protein (17, 29). Relatively few repressor geneslinked to antibiotic biosynthesis loci have been reported, andwhile some of these are implicated as pathway-specific negativeregulators of antibiotic production (8, 62), others controlthe expression of adjacent resistance genes (11, 14) or haveundefined functions (50). Whether PhlF is involved in the regulationof phlE expression remains to beseen.

The phl genes from P. fluorescens Q2-87 define a unique polyketide biosynthetic pathway (Fig. 6) that is conserved among plant-associatedfluorescent pseudomonads (23, 45). The relative simplicityof the locus differs markedly from those of type I and type IIPKSs described previously, although at least some of the biosyntheticreactions involved are likely to be mechanistically similar. Itis especially curious that homologues of phlA, phlC, and phlBare found in archaebacterial genomes but not (at least until now)in eubacteria, whereas phlD homologues are present in the eubacterialgenomes of Bacillus and Mycobacterium as well as in plants. Thisunusual assemblage of phl genes, apparently from different sources,may have arisen due to the nature of the reaction being catalyzed.Plant CHSs use aromatic products of the phenylpropanoid pathwayas primers, and the requirement in bacteria for a simpler, possiblylinear primer molecule may have led to the recruitment of theother three genes in the operon. To our knowledge this is theonly report of such a combination of genes for the synthesis ofa polyketide antibiotic. The requirement of all four proteinsfor the synthesis of MAPG and of PhlA, PhlC, and PhlB for theconversion of MAPG to 2,4-DAPG suggests that these proteins functionas a complex to facilitate substrate transferreactions.

	ACKNOWLEDGMENTS

M. G. Bangera gratefully acknowledges the receipt of a grant from the Storkan/Hanes Research Foundation. This work was supportedby grant 96-35303-3242 from the U.S. Department of Agriculture,Office of Grants and Program Systems, National Research Initiative,Competitive GrantsProgram.

We thank David Weller for providing Pseudomonas strains and Penny von Wettstein-Knowles, Mads Siggaard-Andersen, and AndreaGargas for critical review of the manuscript. We thank Steve Thompsonfor help with sequence analysis, Robert Bonsall for assistancewith HPLC analysis and Dmitri Mavrodi for technicaladvice.

	FOOTNOTES

^* Corresponding author. Mailing address: USDA Agricultural Research Service, Root Disease and Biological Control Research Unit,Washington State University, P.O. Box 646430, Pullman, WA 99164-6430.Phone: (509) 335-0930. Fax: (509) 335-7674. E-mail: thomasho{at}mail.wsu.edu.

Present address: Department of Microbiology, University of Washington, Seattle, WA 98195-7242.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Appel, R. D., A. Bairoch, and D. F. Hochstrasser. 1994. A new generation of information retrieval tools for biologists: the example of the ExPASy WWW server. Trends Biochem. Sci. 19:258-260[Medline].

2. Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1992. Short protocols in molecular biology, p. 16.8-16.9. John Wiley and Sons, New York, N.Y.

3. Bangera, M. G., and L. S. Thomashow. 1996. Characterization of a genomic locus required for synthesis of the antibiotic 2,4-diacetylphloroglucinol by the biological control agent Pseudomonas fluorescens Q2-87. Mol. Plant-Microbe Interact. 9:83-90[Medline].

4. Bangera, M. G., D. M. Weller, and L. S. Thomashow. 1994. Genetic analysis of the 2,4-diacetylphloroglucinol biosynthetic locus from Pseudomonas fluorescens Q2-87, 383-386. In M. J. Daniels, J. A. Downie, and A. E. Osbourn (ed.), Advances in molecular genetics of plant-microbe interactions, vol. 3. Kluwer Academic Publishers, Dordrecht, The Netherlands.

5. Birnboim, H. C., and J. Doly. 1979. A rapid alkaline extraction procedure for screening recombinant plasmid DNA. Nucleic Acids Res. 7:1513-1523[Abstract/Free Full Text].

6. Bonsall, R. F., D. M. Weller, and L. S. Thomashow. 1997. Quantification of 2,4-diacetylphloroglucinol produced by fluorescent Pseudomonas spp. in vitro and in the rhizosphere of wheat. Appl. Environ. Microbiol. 63:951-955[Abstract].

7. Bult, C. J., O. White, G. J. Olsen, L. Zhou, R. D. Fleischmann, G. G. Sutton, J. A. Blake, L. M. Fitzgerald, R. A. Clayton, J. D. Gocayne, A. R. Kerlavage, B. A. Dougherty, J.-F. Tomb, M. D. Adams, C. I. Reich, R. Overbeek, E. F. Kirkness, K. G. Weinstock, J. M. Merrick, A. Glodek, J. L. Scott, N. S. M. Geoghagen, J. F. Weidman, J. L. Fuhrmann, D. Nguyen, T. R. Utterback, J. M. Kelley, J. D. Peterson, P. W. Sadow, M. C. Hanna, M. D. Cotton, K. M. Roberts, M. A. Hurst, B. P. Kaine, M. Borodovsky, H.-P. Klenk, C. M. Fraser, H. O. Smith, C. R. Woese, and J. C. Venter. 1996. Complete genome sequence of the methanogenic archaeon, Methanococcus jannaschii. Science 273:1058-1073[Abstract].

8. Chater, K. F., and M. J. Bibb. 1997. Regulation of bacterial antibiotic production, p. 57-105. In H. Kleinkauf, and H. von Döhren (ed.), Biotechnology, vol. 6. Products of secondary metabolism. VCH, Weinheim, Germany.

9. Cook, R. J., L. S. Thomashow, D. M. Weller, D. Fujimoto, M. Mazzola, G. Bangera, and D.-S. Kim. 1995. Molecular mechanisms of defense by rhizobacteria against root disease. Proc. Natl. Acad. Sci. USA 92:4197-4201[Abstract/Free Full Text].

10. Donadio, S., M. J. Staverm, J. B. McAlpine, S. J. Swanson, and L. Katz. 1991. Modular organization of genes required for complex polyketide biosynthesis. Science 252:675-679[Abstract/Free Full Text].

11. Fernández-Moreno, M. A., J. L. Caballero, D. A. Hopwood, and F. Malpartida. 1991. The act cluster contains regulatory and antibiotic export genes, direct targets for translational control by the bldA tRNA of Streptomyces. Cell 66:769-780[Medline].

12. Fliegmann, J., G. Schröder, S. Schanz, L. Britsch, and J. Schröder. 1992. Molecular analysis of chalcone and dihydropinosylvin synthase from Scots pine (Pinus sylvestris) and differential regulation of these and related enzyme activities in stressed plants. Plant Mol. Biol. 18:489-503[Medline].

13. Genetics Computer Group. 1994. Program manual for the Wisconsin package, version 8. Genetics Computer Group, Madison, Wis.

14. Guilfoile, P. G., and C. R. Hutchinson. 1992. Sequence and transcriptional analysis of the Streptomyces glaucescens tcmAR tetracenomycin C resistance and repressor gene loci. J. Bacteriol. 174:3651-3658[Abstract/Free Full Text].

15. Hamdan, H., D. M. Weller, and L. S. Thomashow. 1991. Relative importance of fluorescent siderophores and other factors in biological control of Gaeumannomyces graminis var. tritici by Pseudomonas fluorescens 2-79 and M4-80R. Appl. Environ. Microbiol. 57:3270-3277[Abstract/Free Full Text].

16. Harrison, L. A., L. Letendre, P. Kovacevich, E. A. Pierson, and D. M. Weller. 1993. Purification of an antibiotic effective against Gaeumannomyces graminis var. tritici produced by a biocontrol agent, Pseudomonas aureofaciens. Soil Biol. Biochem. 25:215-221.

17. Heuer, C., R. K. Hickman, M. S. Curiale, W. Hillen, and S. B. Levy. 1987. Constitutive expression of tetracycline resistance mediated by a Tn10-like element in Haemophilus parainfluenzae results from a mutation in the repressor gene. J. Bacteriol. 169:990-994[Abstract/Free Full Text].

18. Hopwood, D. A., and D. H. Sherman. 1990. Molecular genetics of polyketides and its comparison to fatty acid biosynthesis. Annu. Rev. Genet. 24:37-66[Medline].

19. Hrazdina, G., F. Kreuzaler, K. Halbrock, and H. Grisebach. 1976. Substrate specificity of flavonone synthetase from cell suspension cultures of parsley and structure of release products in vitro. Arch. Biochem. Biophys. 175:392-399[Medline].

20. Hutchinson, C. R., and I. Fujii. 1995. Polyketide synthase gene manipulation: a structure-function approach in engineering novel antibiotics. Annu. Rev. Microbiol. 49:201-238[Medline].

21. Jaworski, J. G., M. A. Post-Beittenmiller, and J. B. Ohlrogge. 1989. Site-directed mutagenesis of the spinach acyl carrier protein-I prosthetic group attachment site. Eur. J. Biochem. 184:603-609[Medline].

22. Katz, L., and S. Donadio. 1993. Polyketide synthesis: prospects for hybrid antibiotics. Annu. Rev. Microbiol. 47:875-912[Medline].

23. Keel, C., D. M. Weller, A. Natsch, G. Défago, R. J. Cook, and L. S. Thomashow. 1996. Conservation of the 2,4-diacetylphloroglucinol biosynthesis locus among fluorescent Pseudomonas strains from diverse geographic locations. Appl. Environ. Microbiol. 62:552-563[Abstract].

24. Kim, D.-S., R. F. Bonsall, L. S. Thomashow, and D. M. Weller. 1995. Construction of transgenic Pseudomonas fluorescens Q69c-80 for improved biocontrol activity to take-all. Phytopathology 85:1146.

25. Kletzin, A., and M. W. W. Adams. 1996. Molecular and phylogenetic characterization of pyruvate and 2-ketoisovalerate ferredoxin oxidoreductases from Pyrococcus furiosus and pyruvate ferredoxin oxidoreductase from Thermotoga maritima. J. Bacteriol. 178:248-257[Abstract/Free Full Text].

26. Lanz, T., S. Tropf, F.-J. Marner, J. Schröder, and G. Schröder. 1991. The role of cysteines in polyketide synthases. J. Biol. Chem. 266:9971-9976[Abstract/Free Full Text].

27. Liyanage, H., D. A. Palmer, U. Ullrich, and C. L. Bender. 1995. Characterization and transcriptional analysis of the gene cluster for coronafacic acid, the polyketide component of the phytotoxin coronatine. Appl. Environ. Microbiol. 61:3843-3848[Abstract].

28. Marsh, J. L., M. Erfle, and E. J. Wykes. 1984. The pIC plasmid and phage vectors with versatile cloning sites for recombinant selection by insertional inactivation. Gene 32:481-485[Medline].

29. Marshall, B., S. Morrissey, P. Flynn, and S. B. Levy. 1986. A new tetracycline-resistance determinant, class E, isolated from Enterobacteriaceae. Gene 50:111-117[Medline].

30. Martin, C. R. 1993. Structure, function, and regulation of chalcone synthase. Int. Rev. Cytol. 147:233-283[Medline].

31. McDaniel, R., S. Ebert-Khosla, D. A. Hopwood, and C. Khosla. 1993. Engineered biosynthesis of novel polyketides. Science 262:1546-1550[Abstract/Free Full Text].

32. Moore, J. T., A. Uppal, F. Maley, and G. F. Maley. 1993. Overcoming inclusion body formation in a high-level expression system. Protein Expr. Purif. 4:160-163[Medline].

33. Morrison, D. A. 1979. Transformation and preservation of competent bacterial cells by freezing. Methods Enzymol. 68:326-331[Medline].

34. Nikaido, H. 1994. Prevention of drug access to bacterial targets: permeability barriers and drug efflux. Science 264:382-388[Abstract/Free Full Text].

35. Nowak-Thompson, B., S. J. Gould, and J. E. Loper. 1997. Identification and sequence analysis of the genes encoding a polyketide synthase required for pyoluteorin biosynthesis in Pseudomonas fluorescens Pf-5. Gene 204:17-24[Medline].

36. Ossendorp, B. C., G. P. H. van Heusden, L. J. de Beer, K. Bos, G. L. Schouten, and K. W. A. Wirtz. 1991. Identification of the cDNA clone which encodes the 58-kDa protein containing the amino acid sequence of rat liver non-specific lipid-transfer protein (sterol-carrier protein 2). Eur. J. Biochem. 201:233-239[Medline].

37. Palmer, M. A. J., E. Differding, R. Gamboni, S. F. Williams, O. P. Peoples, C. T. Walsh, A. J. Sinskey, and S. Masamune. 1991. Biosynthetic thiolase from Zooglea ramigera: evidence for a mechanism involving cys-378 as the active site base. J. Biol. Chem. 266:8369-8375[Abstract/Free Full Text].

38. Pao, S. S., I. T. Paulsen, and M. H. Saier, Jr. 1998. Major facilitator superfamily. Microbiol. Mol. Biol. Rev. 62:1-34[Abstract/Free Full Text].

39. Paulsen, I. T., M. H. Brown, and R. A. Skurray. 1996. Proton-dependent multidrug efflux pumps. Microbiol. Rev. 60:575-608[Abstract/Free Full Text].

40. Penfold, C. N., C. L. Bender, and J. G. Turner. 1996. Characterisation of genes involved in biosynthesis of coronafacic acid, the polyketide component of the phytotoxin coronatine. Gene 183:167-172[Medline].

41. Pfeiffer, S. M., E. E. Furth, T. Ohba, Y. J. Chang, H. Rennert, N. Sakuragi, J. T. Billheimer, and J. F. Strauss, III. 1993. Sterol carrier protein 2: a role in steroid hormone synthesis? J. Steroid Biochem. 47:167-172.

42. Pierson, E. A., and D. M. Weller. 1994. Use of mixtures of fluorescent pseudomonads to suppress take-all and improve the growth of wheat. Phytopathology 84:940-947.

43. Raaijmakers, J. M., R. F. Bonsall, and D. M. Weller. Effect of population density of Pseudomonas fluorescens on production of 2,4-diacetylphloroglucinol in the rhizosphere of wheat. Phytopathology, in press.

44. Raaijmakers, J. M., and D. M. Weller. 1998. Natural plant protection by 2,4-diacetylphloroglucinol-producing Pseudomonas spp. in take-all decline soils. Mol. Plant-Microbe Interact. 11:144-152.

45. Raaijmakers, J. M., D. M. Weller, and L. S. Thomashow. 1997. Frequency of antibiotic producing Pseudomonas spp. in natural environments. Appl. Environ. Microbiol. 63:881-887[Abstract].

46. Rangaswamy, V., R. Mitchell, M. Ullrich, and C. Bender. 1998. Analysis of genes involved in biosynthesis of coronafacic acid, the polyketide component of the phytotoxin coronatine. J. Bacteriol. 180:3330-3338[Abstract/Free Full Text].

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

48. Schröder, J., and G. Schröder. 1990. Stilbene and chalcone synthases: related enzymes with key functions in plant-specific pathways. Z. Naturforsch. Sect. C 45:1-8.

49. Schüz, R., W. Heller, and K. Hahlbrock. 1983. Substrate specificity of chalcone synthase from Petroselinum hortense. J. Biol. Chem. 58:6730-6734.

50. Schwecke, T., J. F. Aparicio, I. Molnar, A. König, L. E. Khaw, S. F. Haydock, M. Oliynyk, P. Caffrey, J. Cortés, J. B. Lester, G. Böhm, J. Staunton, and P. F. Leadlay. 1995. The biosynthetic gene cluster for the polyketide immunosuppressant rapamycin. Proc. Natl. Acad. Sci. USA 92:7839-7843[Abstract/Free Full Text].

51. Seedorf, U., P. Brysch, T. Engel, K. Schrag, and G. Assmann. 1994. Sterol carrier protein X is peroxisomal 3-oxoacyl coenzyme A thiolase with intrinsic sterol carrier and lipid transfer activity. J. Biol. Chem. 269:21277-21283[Abstract/Free Full Text].

52. Shanahan, P., J. D. Glennon, J. J. Crowley, D. F. Donnelly, and F. O'Gara. 1993. Liquid chromatographic assay of microbially derived phloroglucinol antibiotics for establishing the biosynthetic route to production, and the factors affecting their regulation. Anal. Chim. Acta 272:271-277.

53. Siggaard-Andersen, M. 1993. Conserved residues in condensing enzyme domains of fatty acid synthases and related sequences. Protein Seq. Data Anal. 3:325-335.

54. Studier, F. W., A. H. Rosenberg, J. J. Dunn, and J. W. Dubendorff. 1990. Use of the T7 RNA polymerase to direct the expression of cloned genes. Methods Enzymol. 185:60-89[Medline].

55. Tabor, S., and C. C. Richardson. 1985. A bacteriophage T7 RNA polymerase/promoter system for controlled exclusive expression of specific genes. Proc. Natl. Acad. Sci. USA 82:1074-1078[Abstract/Free Full Text].

56. Tautz, D., and M. Renz. 1983. An optimized freeze-squeeze method for the recovery of DNA fragments from agarose gels. Anal. Biochem. 132:14-19[Medline].

57. Thomashow, L. S., and D. M. Weller. 1995. Current concepts in the use of introduced bacteria for biological disease control: mechanisms and antifungal metabolites, p. 187-235. In G. Stacey, and N. Keen (ed.), Plant-Microbe Interactions, vol. 1. Chapman & Hall, New York, N.Y.

58. Tropf, S., B. Kärcher, G. Schröder, and J. Schröder. 1995. Reaction mechanisms of homodimeric plant polyketide synthases (stilbene and chalcone synthase). J. Biol. Chem. 270:7922-7928[Abstract/Free Full Text].

59. Tsay, J.-T., W. Ob, T. J. Larson, S. Jackowski, and C. O. Rock. 1992. Isolation and characterization of the $beta$ -ketoacyl-acyl carrier protein synthase gene (fabH) from Escherichia coli K-12. J. Biol. Chem. 267:6807-6814[Abstract/Free Full Text].

60. Ueda, K., K.-M. Kim, T. Beppu, and S. Horinouchi. 1995. Overexpression of a gene cluster encoding a chalcone synthase-like protein confers redbrown pigment production in Streptomyces griseus. J. Antibiot. 48:638-646[Medline].

61. Vincent, M. N., L. A. Harrison, J. M. Brackin, P. A. Kovacevich, P. Mukerji, D. M. Weller, and E. A. Pierson. 1991. Genetic analysis of the antifungal activity of a soilborne Pseudomonas aureofaciens strain. Appl. Environ. Microbiol. 57:2928-2934[Abstract/Free Full Text].

62. Yang, K., L. Han, and L. C. Vining. 1995. Regulation of jadomycin B production in Streptomyces venezuelae ISP5230: involvement of a repressor gene, jadR₂. J. Bacteriol. 177:6111-6117[Abstract/Free Full Text].

63. Yoshida, H., M. Bogaki, S. Nakamura, K. Ubukata, and M. Konno. 1990. Nucleotide sequence and characterization of the Staphylococcus aureus norA gene, which confers resistance to quinolones. J. Bacteriol. 172:6942-6949[Abstract/Free Full Text].

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Brodhagen, M., Henkels, M. D., Loper, J. E. (2004). Positive Autoregulation and Signaling Properties of Pyoluteorin, an Antibiotic Produced by the Biological Control Organism Pseudomonas fluorescens Pf-5. Appl. Environ. Microbiol. 70: 1758-1766 [Abstract] [Full Text]
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Saxena, P., Yadav, G., Mohanty, D., Gokhale, R. S. (2003). A New Family of Type III Polyketide Synthases in Mycobacterium tuberculosis. J. Biol. Chem. 278: 44780-44790 [Abstract] [Full Text]
Bode, H. B., Muller, R. (2003). Possibility of Bacterial Recruitment of Plant Genes Associated with the Biosynthesis of Secondary Metabolites. Plant Physiol. 132: 1153-1161 [Full Text]
Nowak-Thompson, B., Hammer, P. E., Hill, D. S., Stafford, J., Torkewitz, N., Gaffney, T. D., Lam, S. T., Molnar, I., Ligon, J. M. (2003). 2,5-Dialkylresorcinol Biosynthesis in Pseudomonas aurantiaca: Novel Head-to-Head Condensation of Two Fatty Acid-Derived Precursors. J. Bacteriol. 185: 860-869 [Abstract] [Full Text]
Landa, B. B., Mavrodi, O. V., Raaijmakers, J. M., McSpadden Gardener, B. B., Thomashow, L. S., Weller, D. M. (2002). Differential Ability of Genotypes of 2,4-Diacetylphloroglucinol-Producing Pseudomonas fluorescens Strains To Colonize the Roots of Pea Plants. Appl. Environ. Microbiol. 68: 3226-3237 [Abstract] [Full Text]
Abbas, A., Morrissey, J. P., Marquez, P. C., Sheehan, M. M., Delany, I. R., O'Gara, F. (2002). Characterization of Interactions between the Transcriptional Repressor PhlF and Its Binding Site at the phlA Promoter in Pseudomonas fluorescens F113. J. Bacteriol. 184: 3008-3016 [Abstract] [Full Text]
Notz, R., Maurhofer, M., Dubach, H., Haas, D., Defago, G. (2002). Fusaric Acid-Producing Strains of Fusarium oxysporum Alter 2,4-Diacetylphloroglucinol Biosynthetic Gene Expression in Pseudomonas fluorescens CHA0 In Vitro and in the Rhizosphere of Wheat. Appl. Environ. Microbiol. 68: 2229-2235 [Abstract] [Full Text]
Funa, N., Ohnishi, Y., Ebizuka, Y., Horinouchi, S. (2002). Properties and Substrate Specificity of RppA, a Chalcone Synthase-related Polyketide Synthase in Streptomyces griseus. J. Biol. Chem. 277: 4628-4635 [Abstract] [Full Text]
McSpadden Gardener, B. B., Weller, D. M. (2001). Changes in Populations of Rhizosphere Bacteria Associated with Take-All Disease of Wheat. Appl. Environ. Microbiol. 67: 4414-4425 [Abstract] [Full Text]
Omura, S., Ikeda, H., Ishikawa, J., Hanamoto, A., Takahashi, C., Shinose, M., Takahashi, Y., Horikawa, H., Nakazawa, H., Osonoe, T., Kikuchi, H., Shiba, T., Sakaki, Y., Hattori, M. (2001). Genome sequence of an industrial microorganism Streptomyces avermitilis: Deducing the ability of producing secondary metabolites. Proc. Natl. Acad. Sci. USA 10.1073/pnas.211433198v1 [Abstract] [Full Text]
Dunne, C., Moënne-Loccoz, Y., de Bruijn, F. J., O’Gara, F. (2000). Overproduction of an inducible extracellular serine protease improves biological control of Pythium ultimum by Stenotrophomonas maltophilia strain W81. Microbiology 146: 2069-2078 [Abstract] [Full Text]
McSpadden Gardener, B. B., Schroeder, K. L., Kalloger, S. E., Raaijmakers, J. M., Thomashow, L. S., Weller, D. M. (2000). Genotypic and Phenotypic Diversity of phlD-Containing Pseudomonas Strains Isolated from the Rhizosphere of Wheat. Appl. Environ. Microbiol. 66: 1939-1946 [Abstract] [Full Text]
Schnider-Keel, U., Seematter, A., Maurhofer, M., Blumer, C., Duffy, B., Gigot-Bonnefoy, C., Reimmann, C., Notz, R., Défago, G., Haas, D., Keel, C. (2000). Autoinduction of 2,4-Diacetylphloroglucinol Biosynthesis in the Biocontrol Agent Pseudomonas fluorescens CHA0 and Repression by the Bacterial Metabolites Salicylate and Pyoluteorin. J. Bacteriol. 182: 1215-1225 [Abstract] [Full Text]
Omura, S., Ikeda, H., Ishikawa, J., Hanamoto, A., Takahashi, C., Shinose, M., Takahashi, Y., Horikawa, H., Nakazawa, H., Osonoe, T., Kikuchi, H., Shiba, T., Sakaki, Y., Hattori, M. (2001). Genome sequence of an industrial microorganism Streptomyces avermitilis: Deducing the ability of producing secondary metabolites. Proc. Natl. Acad. Sci. USA 98: 12215-12220 [Abstract] [Full Text]

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1.	Appel, R. D., A. Bairoch, and D. F. Hochstrasser. 1994. A new generation of information retrieval tools for biologists: the example of the ExPASy WWW server. Trends Biochem. Sci. 19:258-260[Medline].
2.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1992. Short protocols in molecular biology, p. 16.8-16.9. John Wiley and Sons, New York, N.Y.
3.	Bangera, M. G., and L. S. Thomashow. 1996. Characterization of a genomic locus required for synthesis of the antibiotic 2,4-diacetylphloroglucinol by the biological control agent Pseudomonas fluorescens Q2-87. Mol. Plant-Microbe Interact. 9:83-90[Medline].
4.	Bangera, M. G., D. M. Weller, and L. S. Thomashow. 1994. Genetic analysis of the 2,4-diacetylphloroglucinol biosynthetic locus from Pseudomonas fluorescens Q2-87, 383-386. In M. J. Daniels, J. A. Downie, and A. E. Osbourn (ed.), Advances in molecular genetics of plant-microbe interactions, vol. 3. Kluwer Academic Publishers, Dordrecht, The Netherlands.
5.	Birnboim, H. C., and J. Doly. 1979. A rapid alkaline extraction procedure for screening recombinant plasmid DNA. Nucleic Acids Res. 7:1513-1523[Abstract/Free Full Text].
6.	Bonsall, R. F., D. M. Weller, and L. S. Thomashow. 1997. Quantification of 2,4-diacetylphloroglucinol produced by fluorescent Pseudomonas spp. in vitro and in the rhizosphere of wheat. Appl. Environ. Microbiol. 63:951-955[Abstract].
7.	Bult, C. J., O. White, G. J. Olsen, L. Zhou, R. D. Fleischmann, G. G. Sutton, J. A. Blake, L. M. Fitzgerald, R. A. Clayton, J. D. Gocayne, A. R. Kerlavage, B. A. Dougherty, J.-F. Tomb, M. D. Adams, C. I. Reich, R. Overbeek, E. F. Kirkness, K. G. Weinstock, J. M. Merrick, A. Glodek, J. L. Scott, N. S. M. Geoghagen, J. F. Weidman, J. L. Fuhrmann, D. Nguyen, T. R. Utterback, J. M. Kelley, J. D. Peterson, P. W. Sadow, M. C. Hanna, M. D. Cotton, K. M. Roberts, M. A. Hurst, B. P. Kaine, M. Borodovsky, H.-P. Klenk, C. M. Fraser, H. O. Smith, C. R. Woese, and J. C. Venter. 1996. Complete genome sequence of the methanogenic archaeon, Methanococcus jannaschii. Science 273:1058-1073[Abstract].
8.	Chater, K. F., and M. J. Bibb. 1997. Regulation of bacterial antibiotic production, p. 57-105. In H. Kleinkauf, and H. von Döhren (ed.), Biotechnology, vol. 6. Products of secondary metabolism. VCH, Weinheim, Germany.
9.	Cook, R. J., L. S. Thomashow, D. M. Weller, D. Fujimoto, M. Mazzola, G. Bangera, and D.-S. Kim. 1995. Molecular mechanisms of defense by rhizobacteria against root disease. Proc. Natl. Acad. Sci. USA 92:4197-4201[Abstract/Free Full Text].
10.	Donadio, S., M. J. Staverm, J. B. McAlpine, S. J. Swanson, and L. Katz. 1991. Modular organization of genes required for complex polyketide biosynthesis. Science 252:675-679[Abstract/Free Full Text].
11.	Fernández-Moreno, M. A., J. L. Caballero, D. A. Hopwood, and F. Malpartida. 1991. The act cluster contains regulatory and antibiotic export genes, direct targets for translational control by the bldA tRNA of Streptomyces. Cell 66:769-780[Medline].
12.	Fliegmann, J., G. Schröder, S. Schanz, L. Britsch, and J. Schröder. 1992. Molecular analysis of chalcone and dihydropinosylvin synthase from Scots pine (Pinus sylvestris) and differential regulation of these and related enzyme activities in stressed plants. Plant Mol. Biol. 18:489-503[Medline].
13.	Genetics Computer Group. 1994. Program manual for the Wisconsin package, version 8. Genetics Computer Group, Madison, Wis.
14.	Guilfoile, P. G., and C. R. Hutchinson. 1992. Sequence and transcriptional analysis of the Streptomyces glaucescens tcmAR tetracenomycin C resistance and repressor gene loci. J. Bacteriol. 174:3651-3658[Abstract/Free Full Text].
15.	Hamdan, H., D. M. Weller, and L. S. Thomashow. 1991. Relative importance of fluorescent siderophores and other factors in biological control of Gaeumannomyces graminis var. tritici by Pseudomonas fluorescens 2-79 and M4-80R. Appl. Environ. Microbiol. 57:3270-3277[Abstract/Free Full Text].
16.	Harrison, L. A., L. Letendre, P. Kovacevich, E. A. Pierson, and D. M. Weller. 1993. Purification of an antibiotic effective against Gaeumannomyces graminis var. tritici produced by a biocontrol agent, Pseudomonas aureofaciens. Soil Biol. Biochem. 25:215-221.
17.	Heuer, C., R. K. Hickman, M. S. Curiale, W. Hillen, and S. B. Levy. 1987. Constitutive expression of tetracycline resistance mediated by a Tn10-like element in Haemophilus parainfluenzae results from a mutation in the repressor gene. J. Bacteriol. 169:990-994[Abstract/Free Full Text].
18.	Hopwood, D. A., and D. H. Sherman. 1990. Molecular genetics of polyketides and its comparison to fatty acid biosynthesis. Annu. Rev. Genet. 24:37-66[Medline].
19.	Hrazdina, G., F. Kreuzaler, K. Halbrock, and H. Grisebach. 1976. Substrate specificity of flavonone synthetase from cell suspension cultures of parsley and structure of release products in vitro. Arch. Biochem. Biophys. 175:392-399[Medline].
20.	Hutchinson, C. R., and I. Fujii. 1995. Polyketide synthase gene manipulation: a structure-function approach in engineering novel antibiotics. Annu. Rev. Microbiol. 49:201-238[Medline].
21.	Jaworski, J. G., M. A. Post-Beittenmiller, and J. B. Ohlrogge. 1989. Site-directed mutagenesis of the spinach acyl carrier protein-I prosthetic group attachment site. Eur. J. Biochem. 184:603-609[Medline].
22.	Katz, L., and S. Donadio. 1993. Polyketide synthesis: prospects for hybrid antibiotics. Annu. Rev. Microbiol. 47:875-912[Medline].
23.	Keel, C., D. M. Weller, A. Natsch, G. Défago, R. J. Cook, and L. S. Thomashow. 1996. Conservation of the 2,4-diacetylphloroglucinol biosynthesis locus among fluorescent Pseudomonas strains from diverse geographic locations. Appl. Environ. Microbiol. 62:552-563[Abstract].
24.	Kim, D.-S., R. F. Bonsall, L. S. Thomashow, and D. M. Weller. 1995. Construction of transgenic Pseudomonas fluorescens Q69c-80 for improved biocontrol activity to take-all. Phytopathology 85:1146.
25.	Kletzin, A., and M. W. W. Adams. 1996. Molecular and phylogenetic characterization of pyruvate and 2-ketoisovalerate ferredoxin oxidoreductases from Pyrococcus furiosus and pyruvate ferredoxin oxidoreductase from Thermotoga maritima. J. Bacteriol. 178:248-257[Abstract/Free Full Text].
26.	Lanz, T., S. Tropf, F.-J. Marner, J. Schröder, and G. Schröder. 1991. The role of cysteines in polyketide synthases. J. Biol. Chem. 266:9971-9976[Abstract/Free Full Text].
27.	Liyanage, H., D. A. Palmer, U. Ullrich, and C. L. Bender. 1995. Characterization and transcriptional analysis of the gene cluster for coronafacic acid, the polyketide component of the phytotoxin coronatine. Appl. Environ. Microbiol. 61:3843-3848[Abstract].
28.	Marsh, J. L., M. Erfle, and E. J. Wykes. 1984. The pIC plasmid and phage vectors with versatile cloning sites for recombinant selection by insertional inactivation. Gene 32:481-485[Medline].
29.	Marshall, B., S. Morrissey, P. Flynn, and S. B. Levy. 1986. A new tetracycline-resistance determinant, class E, isolated from Enterobacteriaceae. Gene 50:111-117[Medline].
30.	Martin, C. R. 1993. Structure, function, and regulation of chalcone synthase. Int. Rev. Cytol. 147:233-283[Medline].
31.	McDaniel, R., S. Ebert-Khosla, D. A. Hopwood, and C. Khosla. 1993. Engineered biosynthesis of novel polyketides. Science 262:1546-1550[Abstract/Free Full Text].
32.	Moore, J. T., A. Uppal, F. Maley, and G. F. Maley. 1993. Overcoming inclusion body formation in a high-level expression system. Protein Expr. Purif. 4:160-163[Medline].
33.	Morrison, D. A. 1979. Transformation and preservation of competent bacterial cells by freezing. Methods Enzymol. 68:326-331[Medline].
34.	Nikaido, H. 1994. Prevention of drug access to bacterial targets: permeability barriers and drug efflux. Science 264:382-388[Abstract/Free Full Text].
35.	Nowak-Thompson, B., S. J. Gould, and J. E. Loper. 1997. Identification and sequence analysis of the genes encoding a polyketide synthase required for pyoluteorin biosynthesis in Pseudomonas fluorescens Pf-5. Gene 204:17-24[Medline].
36.	Ossendorp, B. C., G. P. H. van Heusden, L. J. de Beer, K. Bos, G. L. Schouten, and K. W. A. Wirtz. 1991. Identification of the cDNA clone which encodes the 58-kDa protein containing the amino acid sequence of rat liver non-specific lipid-transfer protein (sterol-carrier protein 2). Eur. J. Biochem. 201:233-239[Medline].
37.	Palmer, M. A. J., E. Differding, R. Gamboni, S. F. Williams, O. P. Peoples, C. T. Walsh, A. J. Sinskey, and S. Masamune. 1991. Biosynthetic thiolase from Zooglea ramigera: evidence for a mechanism involving cys-378 as the active site base. J. Biol. Chem. 266:8369-8375[Abstract/Free Full Text].
38.	Pao, S. S., I. T. Paulsen, and M. H. Saier, Jr. 1998. Major facilitator superfamily. Microbiol. Mol. Biol. Rev. 62:1-34[Abstract/Free Full Text].
39.	Paulsen, I. T., M. H. Brown, and R. A. Skurray. 1996. Proton-dependent multidrug efflux pumps. Microbiol. Rev. 60:575-608[Abstract/Free Full Text].
40.	Penfold, C. N., C. L. Bender, and J. G. Turner. 1996. Characterisation of genes involved in biosynthesis of coronafacic acid, the polyketide component of the phytotoxin coronatine. Gene 183:167-172[Medline].
41.	Pfeiffer, S. M., E. E. Furth, T. Ohba, Y. J. Chang, H. Rennert, N. Sakuragi, J. T. Billheimer, and J. F. Strauss, III. 1993. Sterol carrier protein 2: a role in steroid hormone synthesis? J. Steroid Biochem. 47:167-172.
42.	Pierson, E. A., and D. M. Weller. 1994. Use of mixtures of fluorescent pseudomonads to suppress take-all and improve the growth of wheat. Phytopathology 84:940-947.
43.	Raaijmakers, J. M., R. F. Bonsall, and D. M. Weller. Effect of population density of Pseudomonas fluorescens on production of 2,4-diacetylphloroglucinol in the rhizosphere of wheat. Phytopathology, in press.
44.	Raaijmakers, J. M., and D. M. Weller. 1998. Natural plant protection by 2,4-diacetylphloroglucinol-producing Pseudomonas spp. in take-all decline soils. Mol. Plant-Microbe Interact. 11:144-152.
45.	Raaijmakers, J. M., D. M. Weller, and L. S. Thomashow. 1997. Frequency of antibiotic producing Pseudomonas spp. in natural environments. Appl. Environ. Microbiol. 63:881-887[Abstract].
46.	Rangaswamy, V., R. Mitchell, M. Ullrich, and C. Bender. 1998. Analysis of genes involved in biosynthesis of coronafacic acid, the polyketide component of the phytotoxin coronatine. J. Bacteriol. 180:3330-3338[Abstract/Free Full Text].
47.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring HarborNew York, N.Y..
48.	Schröder, J., and G. Schröder. 1990. Stilbene and chalcone synthases: related enzymes with key functions in plant-specific pathways. Z. Naturforsch. Sect. C 45:1-8.
49.	Schüz, R., W. Heller, and K. Hahlbrock. 1983. Substrate specificity of chalcone synthase from Petroselinum hortense. J. Biol. Chem. 58:6730-6734.
50.	Schwecke, T., J. F. Aparicio, I. Molnar, A. König, L. E. Khaw, S. F. Haydock, M. Oliynyk, P. Caffrey, J. Cortés, J. B. Lester, G. Böhm, J. Staunton, and P. F. Leadlay. 1995. The biosynthetic gene cluster for the polyketide immunosuppressant rapamycin. Proc. Natl. Acad. Sci. USA 92:7839-7843[Abstract/Free Full Text].
51.	Seedorf, U., P. Brysch, T. Engel, K. Schrag, and G. Assmann. 1994. Sterol carrier protein X is peroxisomal 3-oxoacyl coenzyme A thiolase with intrinsic sterol carrier and lipid transfer activity. J. Biol. Chem. 269:21277-21283[Abstract/Free Full Text].
52.	Shanahan, P., J. D. Glennon, J. J. Crowley, D. F. Donnelly, and F. O'Gara. 1993. Liquid chromatographic assay of microbially derived phloroglucinol antibiotics for establishing the biosynthetic route to production, and the factors affecting their regulation. Anal. Chim. Acta 272:271-277.
53.	Siggaard-Andersen, M. 1993. Conserved residues in condensing enzyme domains of fatty acid synthases and related sequences. Protein Seq. Data Anal. 3:325-335.
54.	Studier, F. W., A. H. Rosenberg, J. J. Dunn, and J. W. Dubendorff. 1990. Use of the T7 RNA polymerase to direct the expression of cloned genes. Methods Enzymol. 185:60-89[Medline].
55.	Tabor, S., and C. C. Richardson. 1985. A bacteriophage T7 RNA polymerase/promoter system for controlled exclusive expression of specific genes. Proc. Natl. Acad. Sci. USA 82:1074-1078[Abstract/Free Full Text].
56.	Tautz, D., and M. Renz. 1983. An optimized freeze-squeeze method for the recovery of DNA fragments from agarose gels. Anal. Biochem. 132:14-19[Medline].
57.	Thomashow, L. S., and D. M. Weller. 1995. Current concepts in the use of introduced bacteria for biological disease control: mechanisms and antifungal metabolites, p. 187-235. In G. Stacey, and N. Keen (ed.), Plant-Microbe Interactions, vol. 1. Chapman & Hall, New York, N.Y.
58.	Tropf, S., B. Kärcher, G. Schröder, and J. Schröder. 1995. Reaction mechanisms of homodimeric plant polyketide synthases (stilbene and chalcone synthase). J. Biol. Chem. 270:7922-7928[Abstract/Free Full Text].
59.	Tsay, J.-T., W. Ob, T. J. Larson, S. Jackowski, and C. O. Rock. 1992. Isolation and characterization of the $beta$ -ketoacyl-acyl carrier protein synthase gene (fabH) from Escherichia coli K-12. J. Biol. Chem. 267:6807-6814[Abstract/Free Full Text].
60.	Ueda, K., K.-M. Kim, T. Beppu, and S. Horinouchi. 1995. Overexpression of a gene cluster encoding a chalcone synthase-like protein confers redbrown pigment production in Streptomyces griseus. J. Antibiot. 48:638-646[Medline].
61.	Vincent, M. N., L. A. Harrison, J. M. Brackin, P. A. Kovacevich, P. Mukerji, D. M. Weller, and E. A. Pierson. 1991. Genetic analysis of the antifungal activity of a soilborne Pseudomonas aureofaciens strain. Appl. Environ. Microbiol. 57:2928-2934[Abstract/Free Full Text].
62.	Yang, K., L. Han, and L. C. Vining. 1995. Regulation of jadomycin B production in Streptomyces venezuelae ISP5230: involvement of a repressor gene, jadR₂. J. Bacteriol. 177:6111-6117[Abstract/Free Full Text].
63.	Yoshida, H., M. Bogaki, S. Nakamura, K. Ubukata, and M. Konno. 1990. Nucleotide sequence and characterization of the Staphylococcus aureus norA gene, which confers resistance to quinolones. J. Bacteriol. 172:6942-6949[Abstract/Free Full Text].