Xanthomonas campestris pv. campestris gum Mutants: Effects on Xanthan Biosynthesis and Plant Virulence

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J Bacteriol, April 1998, p. 1607-1617, Vol. 180, No. 7
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Xanthomonas campestris pv. campestris gum Mutants: Effects on Xanthan Biosynthesis and Plant Virulence

Federico Katzen,¹^,² Diego U. Ferreiro,¹ Cristian G. Oddo,¹ M. Verónica Ielmini,¹ Anke Becker,² Alfred Pühler,² and Luis Ielpi¹^,^*

Instituto de Investigaciones Bioquímicas Fundación Campomar, Facultad de Ciencias Exactas y Naturales, UBA, and CONICET, (1405) Buenos Aires, Argentina,¹ and Lehrstuhl für Genetik, Universität Bielefeld, D-33501 Bielefeld, Germany²

Received 17 October 1997/Accepted 24 January 1998

	ABSTRACT

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Xanthan is an industrially important exopolysaccharide produced by the phytopathogenic, gram-negative bacterium Xanthomonascampestris pv. campestris. It is composed of polymerized pentasacchariderepeating units which are assembled by the sequential additionof glucose-1-phosphate, glucose, mannose, glucuronic acid, andmannose on a polyprenol phosphate carrier (L. Ielpi, R. O. Couso,and M. A. Dankert, J. Bacteriol. 175:2490-2500, 1993). A clusterof 12 genes in a region designated xpsI or gum has been suggestedto encode proteins involved in the synthesis and polymerizationof the lipid intermediate. However, no experimental evidence supportingthis suggestion has been published. In this work, from the biochemicalanalysis of a defined set of X. campestris gum mutants, we reportexperimental data for assigning functions to the products of thegum genes. We also show that the first step in the assembly ofthe lipid-linked intermediate is severely affected by the combinationof certain gum and non-gum mutations. In addition, we provideevidence that the C-terminal domain of the gumD gene product issufficient for its glucosyl-1-phosphate transferase activity.Finally, we found that alterations in the later stages of xanthanbiosynthesis reduce the aggressiveness of X. campestris againstthe plant.

	INTRODUCTION

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Xanthomonas campestris pv. campestris is a gram-negative bacterium which is a pathogen of cruciferous plants (15). One ofthe products of X. campestris is an extracellular polysaccharidenamed xanthan gum. Because of its rheological properties, xanthanis a useful polymer for a growing list of commercial applications(3). The structure of xanthan consists of a $beta$ -1,4-linked D-glucosebackbone with trisaccharide side chains composed of mannose-( $beta$ -1,4)-glucuronicacid-( $beta$ -1,2)-mannose attached to alternate glucose residues inthe backbone by $alpha$ -1,3 linkages (33). The mannose residues areacetylated and pyruvylated at specific sites but to various degrees(10, 50) (Fig. 1).

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FIG. 1. Organization of the repeating unit of xanthan. The structure of the xanthan repeating unit is according to Jansson et al. (33). The amount of substituents is variable. Some external mannoses contain a second O-acetyl instead of a pyruvyl substituent (50).

The biosynthetic pathway of xanthan comprises five stages: (i) conversion of simple sugars to nucleotidyl derivative precursors,(ii) assembly of pentasaccharide subunits attached to the innermembrane polyprenol phosphate carrier, (iii) addition of acetyland pyruvate groups, (iv) polymerization of pentasaccharide repeatunits, and (v) secretion of the polymer (24, 29, 31, 32).

Chromosomal regions xpsIII, xpsIV, and xpsVI and a 35.3-kb gene cluster are required for the first stage of xanthan biosynthesis(25, 36). These regions comprise gene functions involved inthe biosynthesis of the sugar nucleotide precursors. Proteinsrelated to the subsequent stages of xanthan biosynthesis havebeen proposed to be encoded by the xpsI or gum region (11, 23,54).

The gum region encompasses 16 kb of the X. campestris genome. Nucleotide sequence analysis predicted the presence of 12 openreading frames (gumB to gumM) (GenBank accession no. U22511)(Fig. 2).

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FIG. 2. X. campestris mutant strains generated for gum gene function analysis. Structural map of the X. campestris gum operon showing the organization of the genes as determined by Capage et al. (11), including the modification reported by Becker et al. (8). Transcriptional fusion mutants are represented by single-foot flags; plasmid integration mutants are denoted by double-foot flags. Black flags represent lacZ-aacC1 insertions or plasmid integrations in X. campestris FC2; white flags represent lacZ-aacC1 insertions or plasmid integrations in X. campestris 3192. Relevant restriction sites used for construction of mutant strains are also shown.

Functions for the products of these genes have been proposed (11, 13, 26, 51, 54), but strong experimental supporthas not been presented. The only gum gene characterized by geneticstudies and biochemical analysis is the kpt or gumL gene encodingthe ketal pyruvate transferase enzyme (37).

Although it has been suggested that extracellular enzymes and xanthan are collectively essential for the pathogenicity ofX. campestris, the roles of the individual factors are not fullyunderstood (5). Although a correlation between a gum gene mutationand reduced plant virulence has been recently shown (12), itis not clear whether any specific step in the assembly, decoration,or polymerization of pentasaccharide repeat units is requiredfor plant infection.

In this report, we describe experimental data for the assignment of a biochemical function to every gum gene product. Ourresults are based on the ability of a defined set of X. campestrisgum mutants to synthesize lipid sugar intermediates and a polymerby using previously developed in vitro assays (31). We showthat the first glycosyltransferase activity within the assemblypathway of the pentasaccharide subunit is severely affected bythe inactivation of other genes, and we provide evidence thatthis catalytic activity is located in the C-terminal domain ofthe gumD product. Furthermore, we analyzed the pathogenicity ofseveral gum and non-gum mutant strains to determine how the inactivationof different gum genes may affect plant virulence.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and growth conditions. The strains and plasmids used in this study are listed in Table 1. Escherichia coli strains were grown in Luria-Bertani mediumat 37°C. X. campestris strains were grown in TY (5 g of tryptone,3 g of yeast extract, and 0.7 g of CaCl₂ per liter of H₂O), inmodified M9 medium (36), or in YM medium (25) at 28°C. Antibioticsfrom Sigma (St. Louis, Mo.) were supplemented as required at thefollowing concentrations (in micrograms per milliliter): for X.campestris, gentamicin, 30; kanamycin, 50; rifampin, 100; andtetracycline, 10; for E. coli, gentamicin, 5; kanamycin, 30; ampicillin,100; and tetracycline, 10.

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TABLE 1. Bacterial strains and plasmids used in this work

DNA biochemistry. Plasmid DNA from E. coli was prepared as described by Priefer (42). DNA restriction, agarose gel electrophoresis, cloningprocedures, and Southern hybridizations were carried out in accordancewith established protocols (45). Total DNA from X. campestriswas isolated as described by Meade et al. (38). Transformationof E. coli cells was performed by the method of Morrison (39).Plasmid DNA was introduced into X. campestris cells by electroporationas instructed by Bio-Rad (Richmond, Calif.) or by conjugationas described by Simon (48).

Permeabilized cells, reaction mixtures, and assay procedures. Permeabilized cells were prepared by EDTA treatment of X. campestris cells as described previously (31). The standard reactionmixtures for the synthesis of lipid-linked intermediates contained70 mM Tris-HCl buffer (pH 8.2), 8 mM MgCl₂, permeabilized cells(0.6 to 0.8 mg of protein), UDP-glucose, GDP-mannose, and UDP-glucuronicacid, either labeled or not (UDP-[¹⁴C]glucose, 15.7 µM; UDP-[¹⁴C]glucuronic acid, 17.1 µM; GDP-[¹⁴C]mannose, 15.7 µM; UDP-glucose, 285 µM; UDP-glucuronic acid,285 µM; GDP-mannose, 142 µM). Acetyl coenzyme A (Ac-CoA), 0.7mM, or phosphoenolpyruvate (PEP), 4.3 mM, was added as indicatedlater in the text. Reactions were performed in a total volumeof 70 µl at 20°C for 30 min and stopped by adding 0.2 ml of 70mM Tris-HCl-10 mM EDTA buffer (pH 8.2). The mixtures were vortexedand centrifuged at 6,000 × g for 5 min, and the pellets were resuspendedand washed two times with the same buffer. The combined supernatants,which contain the in vitro polymerization products, were analyzedby gel filtration chromatography on a Bio-Gel A-5m column (30by 0.9 cm) in 0.1 M pyridinium acetate (pH 5). Fractions of 1ml were collected, and the amount of radioactivity was determinedby liquid scintillation. Data were confirmed by changing the labeleddonor or doing duplicate experiments. The washed cell pelletswere each extracted three times with 150 µl of chloroform-methanol-water(1:2:0.3, vol/vol), referred to as the 1203 extract, and the organicphase was subjected to paper chromatography in a solvent systemof ethanol (96%)-ammonium hydroxide (7:3) (solvent A). Alternatively,the glycolipids present in the 1203 extract were mild-acid hydrolyzed(0.01 N HCl, 100°C, 10 min) and subjected to paper chromatographyin a solvent system of either 2-propanol-acetic acid-water (27:4:9)(solvent B) or butanol-pyridine-water (6:4:3) (solvent C). Alternatively,samples were analyzed by paper electrophoresis in a solvent systemof pyridine-acetic acid-water (1:0.04:9) as previously described(37, 41). Under the mild-acid hydrolysis conditions used,only the phosphate linkages are split, releasing the labeled oligosaccharidefrom the unlabeled lipid. Radioactivity was detected with a Packard7201 radiochromatogram scanner (Packard Instrument Co., Rockville,Md.). Deacetylation of oligosaccharides was performed with 60mM NaOH as previously described (32).

Radiochemicals and biochemicals. UDP-[¹⁴C]glucose (300 Ci/mol), UDP-[¹⁴C]glucuronic acid (300 Ci/mol), and GDP-[¹⁴C]mannose (300 Ci/mol) were prepared as described previously (31).UDP-glucose, GDP-mannose, UDP-glucuronic acid, PEP (monopotassiumsalt), and Ac-CoA were purchased from Sigma.

Virulence tests. X. campestris was grown in modified M9 medium until early log phase and washed with 0.9% NaCl. Cabbage (Brassica oleraceacv. Braunschweiger) was grown in a growth chamber at 25°C and75% humidity for 4 weeks. Bacteria (10⁸ CFU) were injected into the petioles of mature leaves, and thesymptoms were rated 10 days after injection on the basis of thefollowing factor scale: 0, no visible effects; 1, chlorosis aroundthe infection site; 2, chlorosis extending from the infectionsite; 3, blackened leaf veins; 4, chlorosis of leaf tissue; 5,death and drying of tissue; 6, complete rotting of the entireleaf. The virulence index was calculated for each strain as aweight ratio of percentages of plants having the same pathogenicityfactor. Each strain was inoculated into at least 10 independentplants. Mock infection was performed by inoculation of modifiedM9 medium into 10 independent plants.

Analysis of nucleotide and protein sequences. The nucleotide and amino acid sequences were analyzed by using the MacVector Sequence Analysis Software (Oxford MolecularLimited). The amino acid sequences deduced from the nucleotidesequences were compared to those in the GenBank database by usingthe BLAST algorithm (1).

	RESULTS

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Construction of a defined set of X. campestris gum mutants. Since gum genes were shown to be encoded by a single transcriptional unit (34), nonpolar gum mutants were constructed bytranscriptional fusion or plasmid integration (Table 1). Transcriptionalfusion mutants were constructed by marker exchange mutagenesisby using the nonpolar, promoterless lacZ-aacC1 interposon insertedin the same direction as the proposed gum open reading frames(34). Plasmid integration gum mutants were constructed by cloningfragments of gum genes into suicide vector pK18mob (46). Inthis case, gum sequences were cloned in the same direction asvector promoters, allowing transcription downstream of the integrationsite. Hybrid plasmids were transferred to X. campestris strains.X. campestris strains with hybrid plasmids integrated into thegenome by single crossover events were selected by use of thevector-encoded antibiotic resistance, and the changes were verifiedby Southern hybridization.

We were unable to mutate the gumB, gumC, gumE, gumJ, and gumM genes in the FC2 strain (Table 1) without further chromosomalrearrangements. This lethality might be due to accumulation ofcertain toxic, lipid-linked intermediates. However, all of thesegenes could be inactivated in strain 3192, which is deficientin UDP-glucose pyrophosphorylase (25). Due to its failure tosynthesize UDP-glucose, mutant 3192 lacks, in vivo, all of thexanthan biosynthetic lipid intermediates. Figure 2 shows the insertionand integration sites for all of the mutants.

Biochemical characterization of lipid-linked intermediates from gum mutant strains generated in a wild-type background. Permeabilized cells were incubated with UDP-glucose, GDP-mannose, and UDP-glucuronic acid, one of them labeled in the sugarmoiety, and processed as described in Materials and Methods. Lipid-linkedxanthan intermediates were extracted, and oligosaccharides releasedfrom the lipid fraction were characterized by descending chromatographyon solvent B (see Materials and Methods). Results are shown inFig. 3. Previous studies have shown that labeled oligosaccharidesreleased from the glycolipid fraction obtained from permeabilizedFC2 cells consisted mainly of pentasaccharide repeating unitsand their pyruvylated or acetylated derivatives (Fig. 3A). Thepentasaccharide repeating unit corresponds to the peak migratingbetween maltopentaose and maltohexaose (31). The acetylatedpentasaccharide and the pyruvylated pentasaccharide migrate likemaltotetraose. The existence of endogenous acetyl and pyruvyldonors was previously reported (31, 32). The fastest-migratingpeak was characterized as glucose. It could arise from eitherglucose diphosphate polyprenol or lipid-bound glucose (see below),which does not seem to participate in xanthan biosynthesis.

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FIG. 3. Lipid-linked intermediates in gum mutant strains. Standard incubations were carried out in the presence of the substrates indicated in each panel. The gum genotype of each strain is indicated. 1203 extracts were treated by mild-acid hydrolysis and submitted to paper chromatography on solvent B as indicated in Materials and Methods. The X. campestris strains used were FC2 (A, G, and J), XcD (B), Xc405M (C), XcH (D), XcK (E), XcI (F), XcF (H and K), XcG (I and L), Xc405B/pCD2 (M), Xc405C/pCD2 (N), Xc405E/pCD2 (O), and Xc405J/pCD2 (P). Glucose (Glc) and maltooligosaccharides (M₂ to M₆) were run as standards. UDP-glc, UDP-glucose; GDP-man, GDP-mannose; UDP-glcA, UDP-glucuronic acid; wt, wild type.

The gumD mutant XcD was the unique mutant strain, generated in a wild-type background, that showed no released labeled oligosaccharideswhen permeabilized cells were labeled with UDP-[¹⁴C]glucose (Fig. 3B). Cells labeled with UDP-[¹⁴C]glucuronic acid or GDP-[¹⁴C]mannose showed similar results (data not shown). The predictedGumD protein is similar to a large group of glycosyl-1-phosphatetransferases. Among others, the gumD product is similar to galactosyl-1-phosphatetransferases WbaP (55) and ExoY (40, 43). WbaP catalyzesthe transfer of galactosyl-1-phosphate from UDP-galactose to undecaprenylphosphate, the first reaction of O-antigen synthesis of Salmonellaenterica serovar typhimurium. In turn, ExoY of Rhizobium meliloticatalyzes the first reaction in the synthesis of the exopolysaccharidesuccinoglycan. Taken together, these data suggest that GumD catalyzesthe transfer of glucosyl-1-phosphate from UDP-glucose to polyprenolphosphate, which is the first step in the biosynthesis of lipidintermediates involved in the synthesis of xanthan (31). Thisfunction was previously termed glycosyltransferase I (54).

Oligosaccharides obtained from gumH strain XcH could be resolved into two components: a compound with the same mobility asthe disaccharide cellobiose and glucose (Fig. 3D). XcH cells labeledwith UDP-[¹⁴C]glucuronic acid or GDP-[¹⁴C]mannose did not incorporate radioactivity into the 1203 extract(data not shown). These results suggest that gumH encodes glycosyltransferaseIII, catalyzing the addition of an $alpha$ -mannosyl residue from GDP-mannoseto cellobiose diphosphopolyprenol to produce mannosyl-( $alpha$ -1,3)-cellobiosediphosphopolyprenol.

Oligosaccharides released from the lipid fraction of gumK strain XcK could be resolved into three species when permeabilizedcells were labeled with UDP-[¹⁴C]glucose (Fig. 3E). The component with a mobility slightly slowerthan that of the maltotriose corresponds to mannosyl-cellobiose.The component having a mobility similar to that of maltose correspondsto acetylated mannosyl-cellobiose (32). After deesterificationwith 60 mM NaOH, this compound yielded mannosyl-cellobiose, confirmingthe presence of the acetyl group (data not shown). Peaks similarin mobility appeared upon the labeling of these cells with GDP-[¹⁴C]mannose, but no radioactivity was detected in 1203 extractsafter the labeling of XcK cells with UDP-[¹⁴C]glucuronic acid (data not shown). The fastest-migrating componentwas characterized as glucose. Hence, the gumK product appearsto be glycosyltransferase IV, which is responsible for the additionof a glucuronic acid residue from UDP-glucuronic acid to mannosyl-( $alpha$ -1,3)-cellobiosediphosphopolyprenol to produce glucuronyl-( $beta$ -1,2)-mannosyl-( $alpha$ -1,3)-cellobiosediphosphopolyprenol.

As shown in Fig. 3F, three compounds were obtained upon the labeling of gumI mutant XcI with UDP-[¹⁴C]glucose. The major compound released from the resulting lipidfraction showed a mobility similar to that of maltotetraose. Thisis the same mobility as that of the already described tetrasaccharide(31). As pointed out above, this mobility is also similar tothat of acetylpentasaccharide. After deesterification with 60mM NaOH, acetylpentasaccharide produced pentasaccharide, witha shift from near maltooligosaccharide M₄ to M₅-M₆, while thecompound from strain XcI remained unaltered. The minor compoundcorresponds to acetylated tetrasaccharide. The presence of theacetyl group was confirmed by deacetylation. After paper chromatographyon solvent B, the mobility of the product was similar to thatof the tetrasaccharide. Both peaks could be reproduced by labelingof permeabilized cells with either GDP-[¹⁴C]mannose or UDP-[¹⁴C]glucuronic acid (data not shown). The fastest-migrating componentwas characterized as glucose. Thus, it seems likely that gumIencodes glycosyltransferase V, which is involved in the transferenceof a $beta$ -mannosyl residue from GDP-mannose to glucuronyl-( $beta$ -1,2)-mannosyl-( $alpha$ -1,3)-cellobiosediphosphopolyprenol to render mannosyl-( $beta$ -1,4)-glucuronyl-( $beta$ -1,2)-mannosyl-( $alpha$ -1,3)-cellobiosediphosphopolyprenol. Although the assignment of glycosyltransferaseV to GumI is in agreement with earlier reports, accumulation ofa lipid-linked tetrasaccharide was not detected previously (51,54).

The radioactive oligosaccharides obtained from gumF and gumG mutants (XcF and XcG, respectively) labeled with GDP-[¹⁴C]mannose in the presence of Ac-CoA could be resolved into twomajor species (Fig. 3H and I, respectively) with the same mobilitiesof the pentasaccharide and acetylated pentasaccharide obtainedfrom FC2 cells (Fig. 3A and G). In contrast, oligosaccharidesreleased from FC2 cells labeled under identical conditions couldbe separated into three compounds (Fig. 3G). Deacetylation ofoligosaccharides showed that these components represent, fromleft to right, pentasaccharide, monoacetylated pentasaccharide,and diacetylated pentasaccharide (data not shown). No clear diacetylatedpentasaccharide unit was observed among the compounds releasedfrom XcF and XcG 1203 extracts (compare panels G, H, and I inFig. 3). These data indicated that strains XcF and XcG are unableto simultaneously acetylate both of the mannoses present in therepeating unit, suggesting that gumF and gumG encode specificO-acetyltransferases. Since acetylation of the inner mannose couldalso occur at the trisaccharide-diphosphate-prenol level (32)we decided to use this trisaccharide acceptor to distinguish whichgene product, GumF or GumG, is responsible for acetylation ofthe inner mannose. Permeabilized FC2 cells incubated in the presenceof UDP-glucose, GDP-[¹⁴C]mannose, and Ac-CoA released two major components from the lipidfraction, identified as mannosyl-cellobiose and acetylated mannosyl-cellobiose(32) (Fig. 3J). Permeabilized XcG cells similarly incubatedshowed the same pattern of oligosaccharides (Fig. 3L), indicatingthat the inner mannose is partially acetylated. On the other hand,permeabilized XcF cells incubated under the same conditions releasedonly mannosyl-cellobiose from the lipid fraction (Fig. 3K). Ineach case, deacetylation of putative acetylmannosyl-cellobiosegave compounds with mobility identical to that of mannosyl-cellobiose(data not shown). These results indicate that gumF encodes anacetyltransferase whose acceptor is the innermost mannose of thelipid-linked pentasaccharide intermediate (acetyltransferase I),while gumG appears to encode a related enzyme in which the acceptoris the external mannose of the same intermediate (acetyltransferaseII).

Two radioactive products appeared in paper electrophoresis upon mild-acid hydrolysis of 1203 extracts of permeabilized FC2cells labeled with UDP-[¹⁴C]glucuronic acid and with the addition of PEP. These compoundswere characterized as pentasaccharide and pyruvylated pentasaccharide(Fig. 4A) (30). The analysis of oligosaccharides released fromgumL mutant strain XcL labeled in the presence of PEP revealedthat this strain is unable to synthesize the pyruvylated intermediatein vitro, as judged by paper electrophoresis (Fig. 4B). Therefore,the simplest hypothesis is that GumL is the ketal pyruvate transferase.

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FIG. 4. Pyruvylation of the lipid-linked intermediate in gumL and wild-type strains. Incubations were performed in the presence of UDP-[¹⁴C]glucuronic acid, GDP-mannose, UDP-glucose, and PEP. Radioactive material released from 1203 extracts by mild-acid hydrolysis was submitted to paper electrophoresis. X. campestris FC2 (A) and XcL (B) were employed. AMP and UMP were added as internal standards.

Analysis of the lipid-linked compounds produced in vitro by gum mutants generated in a UDP-glucose-deficient background: glucosyl-1-phosphate transferase is severely affected under certain conditions. Permeabilized ugp-gumM cells (Xc405M) labeled with UDP-[¹⁴C]glucose incorporated radioactivity into the glycolipid fraction.The single radioactive peak was characterized as glucose by paperchromatography on solvent B (Fig. 3C) and solvent C. The radioactivematerial incorporated into the glycolipid fraction was furtheranalyzed by paper chromatography on solvent A (data not shown)(31). In this alkaline solvent, glucose diphosphate polyprenolis converted to give the 1,2-cyclic phosphate ester of glucose,with a mobility (R_f) of 0.5. Two compounds were observed in aboutsimilar amounts: peak 1, with an R_f of 0.5, and peak 2, with anR_f of 0.9. Peak 2 was partially characterized as a glucose-boundlipid (see below). Peak 1 had the same mobility in paper electrophoresisas the standard 1,2-cyclic phosphate ester of glucose. After hydrolysisat pH 1 and incubation with alkaline phosphatase, this compoundreleased free glucose. From these results, it was assumed thatXc405M cells synthesized glucose diphosphate polyprenol but wereunable to produce cellobiose diphosphate polyprenol. A likelyexplanation for this is that gumM encodes glycosyltransferaseII, which is involved in the addition of a $beta$ -glucosyl residuefrom UDP-glucose to glucose diphosphate polyprenol to producecellobiose diphosphate polyprenol.

Surprisingly, permeabilized ugp-gumB (Xc405B), ugp-gumC (Xc405C), ugp-gumE (Xc405E), and ugp-gumJ (Xc405J) cells incorporatedno radioactivity into the 1203 extract when labeled with UDP-[¹⁴C]glucuronic acid or GDP-[¹⁴C]mannose (data not shown). Upon the labeling of these cells withUDP-[¹⁴C]glucose, radioactivity was detected in the glycolipid fraction.This material was labile to mild-acid treatment, releasing freeglucose when analyzed by paper chromatography or high-pressureliquid chromatography on an Aminex HPX-87H ion exclusion columnas previously described (41). A single compound with an R_f of0.9 was detected by paper chromatography in alkaline solvent A.As pointed out above, an R_f of 0.5 was expected for glucose diphosphatepolyprenol. The absence of a diphosphate bridge between the glucoseand the lipid moiety was reinforced by DEAE-cellulose column chromatographyin 99% methanol performed as previously reported (4). The compoundeluted at 0.14 M ammonium acetate. Under the same conditions,galactose monophosphate polyprenol is eluted at 0.11 M and glucosediphosphate polyprenol is eluted at 0.23 M. These results suggestthat the radioactive compound formed could be a lipid-bound glucosewith only one negative charge. Its function is unknown, and itdoes not seem to participate in xanthan biosynthesis. Taken together,these results suggest that the glucosyl-1-phosphate transferaseactivity was absent in strains Xc405B, Xc405C, Xc405E, and Xc405J.One possible explanation is that inactivation of certain gum geneswithin a strain containing a ugp mutation alters the normal gumbiosynthetic pathway.

To test whether a combination of a gum mutation with a sugar nucleotide deficiency would lead to arrest of the normal gumbiosynthetic pathway, we decided to generate a known glycosyltransferasegum mutation in a background with altered sugar nucleotide levels.Strain 3192 does not produce UDP-glucose (25) but preservesthe ability to produce xanthan and its lipid-linked intermediatesin vitro if sugar nucleotides are exogenously provided (25).Thus, we disrupted the gumK gene in strain 3192, generating strainXc405K. In this case, disruption of gumK was carried out withthe same construction used to obtain gumK strain XcK. PermeabilizedXc405K cells showed no released labeled trisaccharide when labeledwith either UDP-[¹⁴C]glucose or GDP-[¹⁴C]mannose, while strain XcK was able to synthesize trisaccharidediphosphate polyprenol in vitro (data not shown). Similar resultswere obtained upon the generation of an identical gumK mutationin strain 3332, producing strain Xc475K. Strain 3332 is deficientin phosphomannose isomerase; therefore, it does not produce GDP-mannose(25). These results suggest that deficiencies which lead toa lack of UDP-glucose or GDP-mannose, in combination with certaingum mutations, are likely to abolish the assembly of the lipid-linkedintermediates in vitro. The simplest hypothesis is that the firststep in the assembly of pentasaccharide subunits is being affected.The exception appeared when the combination involved the gumMgene.

Restoration of the gum biosynthetic pathway in a UDP-glucose-defective background: glucosyl-1-phosphate transferase activity seems to be located in the C-terminal domain of gumD. If the first reaction is a limiting step in the biosynthesis of xanthan, it could be reversed by increasing levels of glucosyl-1-phosphatetransferase (the gumD product). Whereas some glycosyl-1-phosphatetransferases display homology to GumD along the whole sequence,others appear to be homologous only to its C-terminal portion(40, 43, 55). These data let us hypothesize that the glucosyl-1-phosphatedomain of GumD resides in its C-terminal half. The coding sequencefor the C-terminal portion of GumD was cloned into broad-host-rangevector pRK404 (18), producing plasmid pCD2 (Table 1). Thisplasmid complemented the xanthan defect in the XcD strain, renderingmucoid colonies. These results suggest that the glucosyl-1-phosphatetransferase activity of GumD relies on its C-terminal half. Theability of Xc405K and Xc475K to synthesize trisaccharide diphosphatepolyprenol in vitro was restored by pCD2 (data not shown). Theplasmid also restored the biosynthesis of cellobiose diphosphatepolyprenol in an additional gumH mutant generated in the straincontaining a ugp mutation (data not shown).

Characterization of lipid-linked intermediates in gum mutant strains generated in a UDP-glucose-deficient background in the presence of plasmid pCD2. Plasmid pCD2 was introduced into Xc405B, Xc405C, Xc405E, and Xc405J by conjugation. Permeabilized cells were labeled withUDP-[¹⁴C]glucuronic acid, and the oligosaccharides released from the1203 extract upon mild-acid hydrolysis were analyzed. The radioactiveoligosaccharides showed a pattern similar to that of those obtainedfrom permeabilized FC2 cells (Fig. 3A, M, N, O, and P). Similarresults were obtained upon the labeling of these cells with UDP-[¹⁴C]glucose or GDP-[¹⁴C]mannose. These data indicate that these strains are capableof both synthesizing and decorating the lipid-linked pentasacchariderepeating unit intermediate. These data suggest that the gumB,gumC, gumE, and gumJ products are not related to the biosynthesisof the lipid-linked intermediates of xanthan.

Plasmid pCD2 was also introduced into Xc405M. A biochemical analysis similar to that described for Xc405M revealed that Xc405M/pCD2behaves exactly the same as parental strain Xc405M, indicatingthat the presence of pCD2 does not modify the xanthan biosyntheticpathway in this strain (data not shown).

Assessment of polysaccharide production in gum mutant strains. Previous studies have shown that a radiolabeled polymer obtained by in vitro incubations, upon gel filtration through a Bio-GelA-5m column, coeluted with a sample of authentic xanthan gum obtainedin vivo. This result indicated similar degrees of polymerizationsince both products had the same apparent molecular weight (about4 × 10⁶) (29, 31). Permeabilized cells from all of the strains depictedin Fig. 3 were labeled with UDP-[¹⁴C]glucose, and their aqueous supernatants were filtered througha Bio-Gel A-5m column.

While inactivation of gumD, gumM, and gumH (encoding the first three glycosyltransferases) completely abolished in vitro polymerformation (data not shown), mutations in genes gumK and gumI (encodingthe fourth and fifth glycosyltransferases, respectively) had lesseffect on the amount of in vitro-produced polysaccharide (Fig.5B and C). Therefore, the lipid-linked trisaccharide and the lipid-linkedtetrasaccharide may fulfill the requirements of substrates forpolymerization. It should be noted that introduction of plasmidpCD2 into Xc405M does not allow the strain to synthesize a polymerin vitro (data not shown). Neither pyruvylation nor acetylationis essential for polysaccharide production, since inactivationof gumF, gumG, or gumL does not affect polymerization (Fig. 5A,D, E, and F).

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FIG. 5. Gel filtration of in vitro-synthesized polymer. Incubations were performed and processed as indicated in Materials and Methods, by using UDP-[¹⁴C]glucose as the labeled donor in the presence of UDP-glucuronic acid and GDP-mannose. The gum genotype of each strain is indicated. The aqueous incubation supernatants were filtered through a Bio-Gel A-5m column at a rate of 0.25 ml min¹. Fractions of 1 ml were collected, and the amount of radioactivity was determined by liquid scintillation. X. campestris FC2 (A), XcK (B), XcI (C), XcF (D), XcG (E), XcL (F), and Xc405J/pCD2 (G) are shown. Void and inclusion volumes were 20 and 45 ml, respectively. These results could be reproduced by using UDP-[¹⁴C]glucuronic acid or GDP-[¹⁴C]mannose as the labeled donor. wt, wild type.

Mutant strains with deficiencies in the expression of gene gumB, gumC, or gumE are the only strains that accumulate lipid-linkedpentasaccharide in vitro without producing polymer (data not shown).Consequently, the functions of these genes are probably relatedto processes involved in polymerization. Permeabilized Xc405J/pCD2cells were able to produce polymer in vitro (Fig. 5G). Similarresults were obtained upon the labeling of cells with UDP-[¹⁴C]glucuronic acid or GDP-[¹⁴C]mannose. Considering that this strain has no defect in the assemblyof the lipid-linked pentasaccharide and the polysaccharide producedis large enough to be excluded by Bio-Gel A5m, the function ofthe gumJ product cannot be associated with a particular xanthanbiosynthetic step. It should be noted that our in vitro systemdoes not allow us to detect defects in the xanthan secretion pathway.Therefore, a secretion role for GumJ cannot be ruled out.

Virulence of X. campestris stable mutant strains altered in different steps of xanthan biosynthesis. Phytopathogenicity-related genes in X. campestris have different effects on polysaccharide production. While mutations withinthe rpf cluster (5, 52) or in the clp gene (16) reducepolysaccharide production, hrp mutants showed no alteration inpolymer biosynthesis (2). However, it has not been establishedwhether any specific stage in xanthan biosynthesis is requiredfor plant virulence. To address this question, we analyzed thevirulence of several stable gum mutants, comparing them to pleiotropicstrain 3192 and to strain FC2. Strains containing episomes orchromosomally integrated plasmids were not analyzed, since theyare unstable without selective pressure.

Compared to strain FC2, xanthan nonproducer strains 3192 and XcD exhibited a 50% virulence index reduction (Fig. 6). Whereasthe absence of a pyruvylated lipid-linked pentasaccharide doesnot have any influence on X. campestris pathogenicity, mutantsunable to simultaneously diacetylate the subunit showed slightlyreduced virulence. A similar result was obtained with the gumIstrain. Although this strain is unable to add the second mannoseto the lipid-linked tetrasaccharide, its virulence index is notseverely affected. These results indicate that the polysaccharideparticipates in, but appears not to be essential for, plant infection.

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FIG. 6. Virulence of X. campestris stable gum mutants. The virulence indexes of X. campestris FC2 (B), XcL (C), XcF (D), XcG (E), XcI (F), XcD (G), and 3192 (H) were determined. The relevant genotype of each strain is indicated. Column A shows the results obtained with mock-infected plants. The standard error was less than 20% in all cases. wt, wild type.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Exploration of the genetics of xanthan gum led to the identification of several genetic loci involved in its biosynthesis(6, 23, 25, 27, 36, 53). Among these gene clusters,the gum region was proposed as being responsible for directingthe final assembly of the polymer (11, 13, 24, 51, 54).However, data unequivocally ascribing functions to gum genes arenot readily available in the public domain. In this report, wepresent, for the first time, direct experimental evidence whichallows us to assign biochemical functions to the X. campestrisgum region.

XcD was the only mutant which did not accumulate any xanthan lipid intermediate. This phenotype would be expected for thegene encoding glycosyltransferase I, as well as any gene productinvolved in the regulatory control of the expression of the gumgenes. Since absence of the gumD product does not abolish transcriptionfrom the main promoter of the gum region (34), GumD may notbe responsible for transcription of the gum operon and probablycorresponds to the first step of xanthan biosynthesis. The predictedGumD protein is similar to a large group of bacterial glucosyl-and galactosyl-1-phosphate transferases, suggesting that theyconstitute a new family of proteins (55).

XcD deficiency could be complemented by the C-terminal half of gumD, suggesting that the glucosyl-1-phosphate transferaseactivity of GumD is located in its C-terminal domain. Similarresults were obtained with the wbaP product, which catalyzes thefirst step of O-antigen synthesis (55).

Analysis of the intermediates accumulated in gumM, gumH, gumK, and gumI mutants showed that these genes encode glycosyltransferasesII, III, IV, and V, respectively, in agreement with previous reports(11, 54). The predicted GumM product revealed homology toa variety of proteins probably involved in the transference ofa glycosyl residue to growing lipid-linked oligosaccharides, suchas AceB of Acetobacter xylinum (GenBank accession no. X94217),which is presumably involved in the second step of acetan biosynthesis.It should be noted that acetan and xanthan have similar structures,and the first four reactions in the assembly of each repeatingunit should be catalyzed by a set of similar glycosyltransferases(22, 41). While the predicted GumH protein is similar to alarge family of prokaryotic $alpha$ -mannosyltransferases (19, 41),the GumI and GumK proteins do not display homology to any publishedsequence.

With the analysis of the in vitro acetylation of the lipid-linked intermediates, we were able to ascertain that GumF is anO-acetyltransferase that modifies the inner mannose while GumGdirects acetylation of the outer mannose. The predicted GumF andGumG proteins are 39% identical, and they might be membrane-associatedproteins, as judged by their hydrophobicity plots. Homologoussequences can be found in different gram-negative and gram-positivebacteria, such as S. enterica (GenBank accession no. X60666),Bacillus subtilis (GenBank accession no. Z99111), and R. loti(GenBank accession no. U22899). Similarities among bacterialO-acetyltransferases, including NodX of R. leguminosarum, NolLof R. loti, and GumF of X. campestris, were reported previously(47).

The gene for ketal pyruvate transferase was previously located on a 1.4-kb BamHI fragment of the gum region (37). Sincethe gumL-lacZ fusion in XcL corresponds to the same complementationgroup as the 31313 mutant (37) and both strains share the samephenotype, it seems very likely that the mutation in strain 31313is located in the gumL gene. GumL is 23.7% identical to ketalpyruvate transferase ExoV of R. meliloti (20), which is involvedin the addition of a pyruvate substituent to the terminal glucoseof the side chain of succinoglycan (44). Although, insertionsin exoV seem to be deleterious, gumL mutants are not affectedin growth and produce normal nonpyruvylated polymer levels (datanot shown).

Under our conditions, we have found that functional gumD, gumM, and gumH genes are required for polymerization of lipid-linkedsubunits while gumK, gumI, gumF, gumG, and gumL mutants are ableto produce a labeled polysaccharide. Whereas gumF, gumG, and gumLstrains produced amounts of polymer similar to those producedby the wild type, the gumK strain produced a very low amount ofpolymer in vivo. This product was described and named polytrimer(9). The gumI strain produced about 10% of the polymer amountproduced by the wild-type strain (data not shown).

We have observed that it is not possible to mutate gumB, gumC, gumE, gumJ, and gumM genes within a wild-type background. Deleteriousmutations in genes required for polysaccharide biosynthesis werealso described in R. meliloti (20). Inactivation of these gumgenes could be performed only in strains which also containeda second mutation. However, most of the double mutants obtainedpresented alterations in the gum biosynthetic pathway. Xc405Marose as an exception, and further experiments are needed to explainthis contradictory behavior. This effect could not be reversedby introduction of plasmid pJC440. Plasmid pJC440 complementsthe ugp mutation in strain 3192 (25) but was unable to reestablishthe production of lipid-linked intermediates in vitro in doublemutants (data not shown). On the other hand, introducing additionalcopies of sequences encoding the C-terminal domain of GumD allowedus to detect in vitro lipid-linked intermediates of xanthan. Somethingcomparable occurred in R. meliloti, since inactivation of thenegative regulator ExoR within a specific background increasedthe efficiency of labeling of intermediates (44).

Combined genetic and biochemical approaches resulted in detailed models of the biosynthesis of polymer subunits of many bacterialpolysaccharides. In contrast, much less is known about the polymerizationand export of these macromolecules. Most of the proposed strategiesfor secretion of polysaccharides from different bacteria wereonly suggested by sequence similarities between essential geneproducts. Linkage between polymerization and export processeswas reported in either polysaccharide or O-antigen biosynthesis(44, 56).

Since gumB, gumC, and gumE strains appear to accumulate complete xanthan subunits in vitro but are unable to synthesize polymer,the products of these genes may be needed for polymerization orpolymer export. GumB and GumC display homology to only two proteinswith known functions (Table 2). These sequence similarities,together with our results, let us hypothesize that GumB mightbe involved in polysaccharide translocation, whereas GumC mightbe involved in determination of the degree of polymerization.GumE displays a hydropathic profile very similar to that of R.meliloti protein ExoQ (40), which was proposed to be involvedin the polymerization of high-molecular-weight succinoglycan (21).Taking into account these considerations, together with our results,we can speculate that the gumE product might be directly relatedto the polymerization of xanthan. These three gene products seemto be membrane-associated proteins, as judged by their hydrophobicityplots. Inactivation of any of these three genes in the wild-typestrain was lethal. This lethality can be explained if we presumethat these gene products are part of a membrane complex. Absenceor deficiency of one of them would disrupt the polymerizationprocess, impairing accumulation of lipid-linked intermediates.Elevated amounts of these compounds might be toxic for the cell.Work is in progress to further characterize polymerization intermediatesin gumB, gumC, and gumE strains (28).

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TABLE 2. Similarities between some gum gene products and proteins with verified polysaccharide secretion roles

In contrast, our gumJ mutant produces lipid-linked pentasaccharide subunits in vitro but is able to polymerize them into xanthan.As can be seen in Table 2, GumJ is homologous to the R. melilotiExoT protein. An R. meliloti exoT mutant produces high-molecular-weightsuccinoglycan and octasaccharide subunits in vitro but fails tosynthesize trimers and tetramers of the octasaccharide subunits(21) which are normally produced in the wild-type strain (7).It should be noted that the amount of high-molecular-weight succinoglycanproduced by the exoT mutant was very low compared to that of thepolymer synthesized by the wild-type strain, suggesting that absenceof the ExoT protein also disturbs polysaccharide production. However,reduction of in vitro pentasaccharide subunit or polysaccharideproduction was not observed in strain Xc405J/pCD2 compared tothe wild type (Fig. 3P and 5G). Low-molecular-weight xanthan hasnot been detected in X. campestris cultures. Providing that polymerizationand export of xanthan are coupled events, GumJ might be involvedin a parallel or subsequent stage of these processes. Consideringthat gumJ disruption within a wild-type background was lethal,gumJ might be necessary to prevent accumulation of a harmful productor for recycling of essential substrates. Figure 7 summarizesthe proposed Gum function in the xanthan biosynthetic pathway.

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FIG. 7. Scheme of the proposed gum gene functions for the biosynthesis of the exopolysaccharide xanthan in X. campestris. The components of the lipid-linked intermediates are represented as follows: Glc, glucose; Man, mannose; GlcA, glucuronic acid; Ac, acetyl group; Pyr, pyruvyl group. The designation of each protein is followed by its proposed function as follows: GT, glycosyltransferase; AT, acetyltransferase; KPT, ketal pyruvate transferase. Dashed arrows indicate that repeating units are variably decorated. GumJ could not be associated with any particular gum biosynthetic step, although the possibility of its participation in pre- or postpolymerization processes cannot be eliminated (see text).

All of the mutants described in this report were similar in color. In addition, 1203 extracts exhibited identical absorptionspectrum patterns (not shown), indicating that the ratio of differentxanthomonadins had not changed. These results stand in contrastto those of a recently published report which proposed that theX. campestris gumD gene is involved not only in xanthan biosynthesisbut also in plant virulence and normal cell pigmentation (12).

Since a correlation between xanthan production and plant virulence was established by employing pleiotropic mutants, the participationof xanthan in bacterial pathogenesis must be interpreted cautiously(17). Unless total loss of pathogenicity takes place (ratherthan variance in the aggressiveness of the pathogen), differencesin virulence between strains could be very subtle (14). Therefore,we decided to express bacterial virulence as an index, which involvesthe inspection of a statistically significant number of infectedplants. Xanthan biosynthesis can be blocked at different stepsof the biosynthetic pathway (24). Inactivation of enzymes involvedin the synthesis of sugar nucleotides abolished xanthan productionand has pleiotropic effects, since these enzymes are also involvedin the biosynthesis of cyclic glucans and lipopolysaccharides(36). In contrast, gene disruption within the gum region islikely to abolish enzyme activity restricted to the polysaccharidebiosynthetic pathway.

Figure 6 shows that pyruvylation was the only change in the lipid-linked intermediate, which is absolutely irrelevant to virulence.However, slight variations in xanthan intermediates, like shorteningof the subunit to four sugars or inactivation of acetyltransferases,reduced the virulence index by approximately 25%. In particular,the virulence of two xanthan-deficient strains mutated at differentstages of xanthan biosynthesis was 50% lower than that of thewild-type strain. Taken together, our data show that althoughxanthan gum is not essential for plant virulence, specific changesin the last stages of xanthan biosynthesis point to a reductionof the aggressiveness of X. campestris against the host.

	ACKNOWLEDGMENTS

We thank Nancy E. Harding (Kelco, Unit of Monsanto Co.) for kindly providing X. campestris 3332 and 3192. We also thank SusanaRaffo and Maria de los Angeles Curto for preparing ¹⁴C-labeled compounds, Marta Bravo for technical assistance withhigh-pressure liquid chromatography analysis, Dorothee Steinmannfor assistance with virulence tests, and Gonzalo de Prat Gay forcritically reviewing the manuscript.

F.K. acknowledges Ph.D. grants from Universidad de Buenos Aires, Deutscher Akademischer Austauschdienst, and the DeutscheForschungsgemeinschaft (Sonderforschungbereich 223). This workwas partly supported by grants Ex-240 from Universidad de BuenosAires and PICT 157 from CONICET to L.I. L.I. is member of Carreradel Investigador (CONICET, Buenos Aires, Argentina).

	FOOTNOTES

^* Corresponding author. Mailing address: Instituto de Investigaciones Bioquímicas Fundación Campomar, Patricias Argentinas435, (1405) Buenos Aires, Argentina. Phone: 54(1) 863-4011/19.Fax: 54(1) 865-2246. E-mail: lielpi{at}iris.iib.uba.ar.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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