Multicomponent Transcriptional Regulation at the Complex Promoter of the Exopolysaccharide I Biosynthetic Operon of Ralstonia solanacearum

doi:10.1128/JB.182.23.6659-6666.2000

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Journal of Bacteriology, December 2000, p. 6659-6666, Vol. 182, No. 23
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Multicomponent Transcriptional Regulation at the Complex Promoter of the Exopolysaccharide I Biosynthetic Operon of Ralstonia solanacearum

Ram P. Garg,¹ Jianzhong Huang,¹^, Wandee Yindeeyoungyeon,¹ Timothy P. Denny,² and Mark A. Schell¹^,²^,^*

Department of Microbiology¹ and Department of Plant Pathology,² University of Georgia, Athens, Georgia 30602-2604

Received 18 May 2000/Accepted 6 September 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

High-level transcription of eps, an operon encoding biosynthesis of an exopolysaccharide virulence factor of the phytopathogenRalstonia (Pseudomonas) solanacearum, requires the products ofat least seven regulatory genes (phcA, phcB, xpsR, vsrA-vsrD,and vsrB-vsrC), which are organized in three converging signaltransduction cascades. Because xpsR and the vsrB-vsrC two-componentsystem are the most downstream cascade components required foractivation of eps, we explored how these components control transcriptionfrom the eps promoter (P_eps). Deletion and PCR mutagenesisidentified an upstream region of P_eps (nucleotides $-$ 82to $-$ 62) that is critical for transcription activation by VsrB-VsrCand XpsR and also is required for negative control of P_epsby the putative eps regulator EpsR. Using PCR mutagenesis we generatedthe vsrC1 allele that encodes a response regulator that constitutivelyactivates P_eps in the absence of its cognate sensor,VsrB. However, activation of P_eps by vsrC1 still requiredxpsR. Unexpectedly, the amino acid substitution conferring theconstitutive phenotype on VsrC1 is 12 residues from its C terminus,outside the known functional domains of response regulators. Finally,a modified DNase I footprinting method was used to demonstratespecific binding of both VsrC1 and VsrC to the $-$ 72 to $-$ 62 upstreamregion of P_eps.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Ralstonia (Pseudomonas) solanacearum, which causes a lethal wilting disease of solanaceous and many other types of other plants(15, 16), enters hosts via natural openings or wounds in rootsand then proceeds to extensively colonize xylem vessels of thevascular system (37, 44). Although secreted plant cell wall-degradingexoenzymes enhance virulence (possibly by facilitating invasionand vascular colonization [23, 24, 37]), it is exopolysaccharideI (EPS I), a large, nitrogen-rich, acidic exopolysaccharide (34),that is the primary virulence factor of R. solanacearum. EPS Iis produced in copious amounts and is required for wilting andkilling of hosts (8, 29). EPS I apparently causes wiltingby restricting water flow through xylem vessels (6). It alsomarkedly enhances the speed and extent of stem colonization (37).

In R. solanacearum, production of EPS I (as well as some exoenzymes) is stringently controlled by a cascading network of morethan 10 regulatory genes (5, 11, 20, 41). Inactivationof any of seven genes in this network causes a >85% reductionin transcription from the eps promoter (P_eps), leadingto loss of EPS I production and the ability to wilt and kill.However, inactivation of all but two of these genes (vsrB andvsrC) can be suppressed by constitutive expression of xpsR froma vector promoter (20). These and other data showed that VsrB,VsrC, and XpsR are the most downstream components in the eps regulatorycascade and suggested that they may directly affect interactionof RNA polymerase with P_eps.

The predicted amino acid sequences of VsrB and VsrC imply that they comprise a two-component system in which VsrB is a sensorkinase and VsrC is its cognate response regulator (19, 20).However, no homologs of the very basic XpsR protein have beenfound. How these three proteins interact to control P_epsis not clear. Nonetheless, analogy to other two-component systems(17) implies that, in response to some unknown signal, VsrBphosphorylates VsrC, thereby stimulating it to turn on transcription,possibly via direct binding to P_eps. EpsR, a putativeDNA-binding protein, is another potential regulator of P_eps,since its overproduction strongly represses EPS I synthesis byR. solanacearum strain K60 (18, 25).

Since there was no clear or direct evidence for physical interactions between P_eps and VsrC, XpsR, or EpsR, we firstused deletion and PCR mutagenesis to define an upstream regionof P_eps that is absolutely required for its transcriptionactivation by VsrB-VsrC and XpsR. Then we generated a vsrC allelethat activated P_eps independently of vsrB and used DNaseI footprinting to show that both this constitutively active VsrCprotein and wild-type VsrC directly bind to the region of P_epsthat was identified by mutagenesis to be important in transcriptionactivation. However, since the affinity of VsrC for P_epswas weak and since the constitutively active VsrC protein wasunresponsive to VsrB and still required XpsR for activation ofP_eps, we speculate that XpsR may facilitate or stabilizebinding of VsrC to P_eps.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacteria and plasmids. Most strains and plasmids constructed and used in this work are described in Table 1. R. solanacearum was grown in BG orBSM medium (36) at 30°C, while Escherichia coli was grown inLB (33) at 37°C. The host strain and vectors used for cloningwere E. coli DH5 $alpha$ (14) and pTZ19U/18U (31), respectively.pPF12 (7) and pEPS1 (21) were described previously. R. solanacearumstrain AW22 was constructed by transposon mutagenesis with Tn3lacZ(7). Derivatives of AW22 were constructed by natural transformation(20) with genomic DNA from AW-R164, AW-C, and AW-MG2 (19).Concentrations (micrograms per milliliter) of antibiotics usedto select and maintain plasmids were kanamycin (Km), 50; spectinomycin(Sp), 50; ampicillin (Amp), 100; and tetracycline (Tc), 20.

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TABLE 1. Important R. solanacearum strains and plasmids used

Construction of P_eps reporter plasmids. P_eps fragments with various lengths of upstream sequences were made by PCR using primers EPS1 (5'-CCGGATCCCCAACTGTAAATCGTA-3'),EPS2 (5'-CCGGATCCAAACGAAATATGCATT-3'), EPS3 (5'-CCGGATCCTTTCGGTATTGAAGC-3'),EPS4 (5'-CCGGATCCATGCACAACCGTATC-3'), EPS5 (5'-TCGGATCCATCGCCACCGGTACTG-3'),EPS6 (CCGGATCCAGAACGATCCATGTTTC-3'), EPS7 (5'-CCCCGGGTTGGCGTTCTGCCTAT-3'),EPS9 (5'-GAGGATCCAGTTGCAGAAACGGCCA-3'), M13F (TGTAAAACGACGGCCAGT-3'),M13R (5'-AGCGAATAACAATTTCACACAGGA-3'), and T7 (5'-TAATACGACTCACTATAGGG-3').PCR mixtures (100 µl) contained 10 mM Tris (pH 8.3), 50 mM KCl,1 mM of each deoxynucleoside triphosphate (dNTP), 2 mM MgCl₂,0.1 nmol of primers, 1 to 5 ng of template, and 2 U of Taq polymerase(Perkin-Elmer). Each amplification cycle consisted of denaturationat 94°C for 1 min, annealing at 50°C for 1 min, and extensionat 72°C for 1 min. After 30 cycles, there was a final extensionat 72°C for 10 min. The P_eps DNA fragments from nucleotides $-$ 538 to +23, $-$ 337 to +23, and $-$ 243 to +23 were amplified usingpXPS1 as template and primer pairs EPS6-EPS4, EPS7-EPS4, and EPS9-EPS4,respectively. The P_eps DNA fragments from $-$ 143 to +23, $-$ 101 to +23, $-$ 68 to +23, and $-$ 44 to +23 were amplified using primerpairs M13F-EPS4, EPS1-EPS4, EPS2-EPS4, and EPS3-EPS4, respectively,and pXPS5 as template. PCR products were digested with BamHI and/orSmaI and ligated into the promoterless lacZ fusion vector pRG970(43) digested in the same manner. After transformation intoE. coli and plating on LB agar with Sp and 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside(X-Gal), plasmid DNA was isolated from blue colonies, and theorientation and identity of the insert wereconfirmed.

PCR mutagenesis of P_eps and vsrC. To mutagenize P_eps, sequences between nucleotides $-$ 143 and +23 were PCR amplified essentially as above using a pTZSZ12template. However, the dATP concentration was 0.2 mM instead of1 mM, and MnCl₂ was added to 0.5 mM. BamHI-digested PCR productswere ligated with BamHI-digested pRG970 and transformed into E.coli, and ~10,000 blue-colored transformants arising on LB plateswith Sp and X-Gal were individually picked and pooled, and plasmidDNA was isolated from them. Pooled plasmids were electroporatedinto R. solanacearum strain AW201 (epsA1::nptl). After platingon BG agar with Sp and X-Gal, white or pale-blue transformants(i.e., those with decreased LacZ activity) were observed at 0.3%.Plasmids from these colonies were individually isolated, transformedinto E. coli, reisolated, and analyzed with restriction enzymesto confirm P_eps inserts. Sequence alterations were determinedafter recloning inserts intopTZ19U.

To mutagenize vsrC, PCRs were performed under mutagenic conditions as above, using pKVC3 as template and an M13F-T7 primerpair. After digestion with HindIII and EcoRI, the PCR productswere ligated with similarly digested pTZ19U and transformed intoE. coli. Plasmid DNA was isolated en masse from ~20,000 transformantcolonies that were washed from plates. The vsrC alleles in thisplasmid pool were released by digestion with HindIII and EcoRIand ligated with similarly digested pRK415 (26), followed bytransformation into E. coli. Plasmid DNA was isolated from ~20,000pooled Tc-resistant colonies and electroporated into R. solanacearumstrain AW22B (vsrB:: $Omega$ eps::lacZ). After selection on BG plateswith X-Gal and Tc, transformants showing increased expressionof the eps::lacZ reporter (i.e., darker-blue color) wereanalyzed.

To construct the vsrC2 allele, vsrC sequences between nucleotides 523 and 1,194 (GenBank U18134) were amplified using apRKVC3 template, a T7 primer, and a primer containing vsrC sequencesbetween nucleotides 1,162 and 1,194 but having a C1185T mutation(S209L) and a same-sense C1171G silent mutation that introduceda BamHI site (5'-TCCATGCGCAAGATGATCTGGATCCGCGTGCGC-3'). The resultantPCR product and a plasmid with sequences 1,145 to 1,290 of vsrCwere mixed, and PCR amplification was performed with T7 and M13Fprimers. The 800-bp vsrC PCR product was digested with HindIIIand EcoRI and cloned into pRK415. Plasmids from transformantswere isolated and screened for the introduced BamHI site. ThevsrC allele from one candidate plasmid (pVSRC2) was sequencedto confirm that it contained the S209Lmutation.

Purification of His-tagged VsrC proteins. Wild-type vsrC was PCR amplified using pKVC3 as template and primers M13F and VSRCN (5'-ACGGATCCACGAGCTCGCTGCG-3'; complementaryto sequences encoding the N terminus of VsrC). The product wasdigested with BamHI and cloned in frame to the hexahistidine-encodingtag of BamHI-digested pTrc-HisA (Invitrogen), yielding plasmidpVSRCH. To generate pCB92, the SacI-KpnI fragment of pVSRCH wasreplaced with the analogous fragment frompVSRC1.

E. coli JM109 (45) cells containing pVSRCH or pCB92 were shaken at 37°C in LB plus Amp until the optical density at 600nm (OD₆₀₀) was 0.6. The 100-ml culture was shifted to 28°C, andisopropyl- $beta$ -D-thio-galactoside was added to 0.4 mM. After 18 h,cells were harvested, suspended in 10 ml of buffer B (5 mM imidazole,500 mM NaCl, 20 mM Tris-HCl [pH 8.0]) and sonicated five timesfor 10 s. The sonicate was centrifuged at 30,000 × g for 25 min,and the supernatant was passed through a 3-ml column containing1 ml of Ni-nitriloacetic acid resin (Sigma) equilibrated withbuffer B. The column was washed with 10 ml of buffer B followedby 10 ml of buffer B with 50 mM imidazole. VsrCs were eluted withbuffer B plus 0.5 M imidazole; sodium dodecyl sulfate-polyacrylamidegel electrophoresis indicated >90%purity.

Construction of an epsR null mutant. The epsR homolog of R. solanacearum strain AW was PCR amplified from genomic DNA as above except that annealing and extensionwere at 70°C. Primers (EPSRN, 5'-AAGGATCCAGG CGGCGCAGTG-3' [nucleotides355 through 381 with an added BamHI site] and EPSRC, 5'-ATGAATTCAGCCCGGCGTGCACGAGGCG-3'[nucleotides 1,055 through 1,075 with an added EcoRI site]) werebased on the sequence of epsR from R. solanacearum strain K60(GenBank M61197). The resultant PCR product was digested withBamHI and EcoRI and cloned into pTZ18U. DNA sequencing showedthat epsR from strain AW is >97% identical to epsR from strainK60.

To construct the epsR null mutant, an internal StyI fragment lacking sequences encoding the first 12 N-terminal residues andlast 52 C-terminal residues of EpsR was made blunt ended withT4 DNA polymerase and then cloned into the SmaI site of suicidevector pTOK2 (27). The resultant plasmid (pEPSR-T) was electroporatedinto R. solanacearum AW, and strains in which the plasmid integratedinto epsR by a single recombination event were selected by Tcresistance. Genomic DNA from two strains was prepared and disruptionof the genomic copy of epsR was confirmed by PCR; no PCR productscould be obtained using EPSRN and EPSRC primers, whereas a PCRproduct of the predicted size was obtained with wild-type DNAas template. An EPSRN and M13R vector primer gave a PCR fragmentof the size predicted for the truncated epsRgene.

Measurement of PglA. Assay samples were spotted onto nitrocellulose and after blocking for 2 h at 25°C with 5% skim milk (Difco) in TBS (10 mMTris HCl [pH 7.4], 140 mM NaCl), the membrane was washed threetimes with TBST (TBS with 0.2% Tween 20) and submerged for 1 hin 10 ml of TBST containing a 1:1,000 dilution of anti-PglA antiserum(39). After three washes with TBST, one with TBST containing0.85 M NaCl, and one with TBST, bound PglA antibodies were detectedwith anti-rabbit immunoglobulin G (IgG) conjugated to alkalinephosphatase (Jackson Immunologicals), 5-bromo-4-chloro-3-indolyl-phosphate,and nitroblue tetrazolium (32).

DNase I footprinting. Target DNA fragments were prepared by PCR essentially as described above and previously (46) using 0.2 mM dNTPs, pPSZ17as template, and primers *M13L (5'-[6-FAM]-CACGACGTTGTAAAACGACGGCCAGT-3';PE Applied Biosystems) and T7. The resultant PCR product (containingsequences between $-$ 337 and +23 of P_eps and labeled atone 5' end with the 6-FAM fluorescent tag) was gel purified, and40 ng (10 nM) was used in 10-µl footprinting-reaction mixturesthat contained 10 mM Tris-HCl (pH 7.5), 5 mM KCl, 1 mM EDTA, 8%glycerol, and 0.5 to 4 µm (0.4 to 3.5 µg) of purified His-taggedVsrC proteins. The total protein concentration was maintainedat 4.5 mg/ml using bovine serum albumin. After 30 min at 30°C,reaction mixtures were placed at 26°C, and 5 µl of RNase-freeDNase I (1.2 × 10⁵ U/µl, freshly diluted [Boehringer Mannheim]) were added. After4 min, 15 µl of 0.5 M EDTA (pH 8.0) was added; reactions wereextracted with phenol-chloroform and passed through a CENTRI-SEPcolumn (Princeton Separations). Digestion products were vacuumdried, dissolved in 12 µl of deionized formamide, 0.2 µl of GS-500-ROXsize standards (PE Biosystems) was added, and the fragmentationpatterns were analyzed with an ABI 310 Genetic Analyzer as describedpreviously (46).

General molecular and genetic techniques. Methods for plasmid isolation from E. coli or R. solanacearum and subsequent transfer into E. coli using the CaCl₂-treatedcompetent cells or into R. solanacearum via electroporation weredescribed earlier (21, 22). Restriction enzymes, DNA ligase,Klenow fragment, and other DNA enzymes were used according tothe manufacturer's recommendations. DNA sequences were obtainedusing an ABI 377 sequencer. Other general molecular genetic techniquesused are described elsewhere (1, 28).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Two regions of the eps promoter are involved in its transcriptional activation. To define the extent of upstream sequences that are required for transcriptional activation of P_eps, we constructeda series of reporter plasmids with various lengths of P_epsfused to lacZ. Expression of these reporter genes was assayedin an R. solanacearum wild-type strain and in strains lackingkey regulators. A reporter plasmid with sequences between $-$ 538and +23 of P_eps fused to lacZ(pPSZ15) gave a high levelof P_eps expression that was strongly dependent on bothxpsR and vsrC, since P_eps expression was reduced at least50-fold by inactivation of either regulator (Fig. 1). Deletionof sequences upstream of $-$ 337 or $-$ 243 did not dramatically alterexpression or regulation, indicating that sequences between $-$ 243and +23 are sufficient for wild-type expression from P_eps.When sequences between $-$ 243 and $-$ 143 were deleted (pPSZ12 [Fig.1]), expression was reduced about threefold, suggesting that asite in the region between nucleotides $-$ 243 and $-$ 143 stimulatesP_eps expression. Residual expression from this reporterconstruct, however, remained strongly dependent on both vsrC andxpsR. Deletion of sequences between $-$ 143 and $-$ 101 did not significantlyreduce transcription below that observed with a reporter havingthe $-$ 143 to +23 region of P_eps fused to lacZ. However,when sequences between nucleotides $-$ 101 and $-$ 68 were deleted,P_eps expression was reduced to less than 5% of the levelsobserved with the $-$ 243 to +23 fusion. Expression was only marginallyfurther reduced when P_eps sequences down to $-$ 44 weredeleted (pPSZ22 [Fig. 1]), regardless of the genetic background.These data show that the $-$ 101 to $-$ 68 region contains sequencesthat are absolutely required for activation of P_eps bythese two regulators.

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FIG. 1. Identification of upstream regions involved in transcriptional regulation of P_eps by VsrC and XpsR. The eps promoter and various lengths of upstream sequences were fused to lacZ on pRG970, generating plasmids pPSZ12 through pPSZ22. Plasmids were transferred into R. solanacearum wild-type (WT) strain AW, into strain AW-C, a vsrC mutant, and into strain AW-R164, an xpsR mutant. P_eps expression (i.e., transcription directed by the P_eps fragment) was monitored by measuring LacZ activity (given in Miller units [33]) in cells from cultures grown overnight in BG medium as described previously (4, 20). LacZ activity from cells harboring an empty pRG970 vector was 15. Nucleotide numbering is relative to the transcription start site of eps (21). The hatched boxes indicate the two important regions for activation of eps. The sequence at the top is that of the region identified by PCR mutagenesis as essential for transcription activation by xpsR and vsrC. +, positions of substitution mutations that reduced or eliminated activation of P_eps (see Table 2). Underlined sequences, putative palindromic recognition sequences for VsrC. Values are averages from three experiments with <25% variation.

Determination of nucleotides required for activation and regulation of P_eps. To delineate more precisely the sequences that are critical for P_eps regulation, a fragment with P_eps nucleotides $-$ 143 to +23 was subjected to mutagenic PCR, and the products werejoined to lacZ on pRG970 to generate transcriptional fusions.The resultant pooled reporter constructs were introduced intowild-type R. solanacearum, and colonies were screened for alteredP_eps::lacZ expression by using X-Gal. Sixteenmutant plasmids were obtained and characterized further by DNAsequencing and quantitative LacZ assays (Table 2). P_eps::lacZexpression from plasmids with single-nucleotide substitutionsat P_eps nucleotides $-$ 74, $-$ 71, $-$ 70, and $-$ 69 was reduced~10-fold, almost to the basal levels given by plasmids in whichall upstream activation sequences had been deleted (compare topPSZ22 and pPSZ21 [Fig. 1]). When assayed in xpsR or vsrC mutantsof R. solanacearum, expression directed by these mutant promoterswas only marginally reduced, indicating that these mutations largelyeliminate activation of P_eps transcription by VsrC andXpsR. Fusion plasmids with single nucleotide substitutions atP_eps nucleotides $-$ 82, $-$ 79, $-$ 72, $-$ 68, and $-$ 67 were reducedabout fivefold. However, when assayed in xpsR or vsrC mutant backgroundsof R. solanacearum, P_eps expression from these promoterswas reduced an additional three- to fourfold to basal levels,indicating that these mutant promoters are inefficiently activatedby VsrC and XpsR. In summary, these results suggest that nucleotidesbetween $-$ 82 and $-$ 62, and in particular the sequence GTGGGGAA between $-$ 74 and $-$ 67 (Fig. 1), are important for activation of P_eps.It is plausible that this region contains the binding sites forP_eps activators, perhaps VsrC and/or XpsR.

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TABLE 2. Expression and regulation of mutant eps promoters^a

When P_eps sequences between nucleotides $-$ 538 and $-$ 143 were restored in the proper orientation and position to theP_eps::lacZ fusion plasmids with substitutionsat $-$ 67 or $-$ 72 and the resultant plasmids placed in wild-type R.solanacearum, P_eps expression was largely the same asobserved with shorter ( $-$ 143 to +23) P_eps fragments (Table2 versus Table 3). These results support the conclusion thatthe primary P_eps regulatory sequences required for transcriptionactivation by VsrC and XpsR lie downstream of nucleotide $-$ 143,while sequences upstream of $-$ 143 can only enhance activation bythese regulators.

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TABLE 3. Effect of selected mutations on expression directed by P_eps fragments with different upstream lengths

Three other single-nucleotide substitutions (at nucleotides $-$ 12, $-$ 9, and $-$ 7) also dramatically reduced P_eps expression(Table 2). The position and nature of these mutations are consistentwith the presumed role of this region as the $-$ 10 consensus hexamerof the promoter (21). A single-nucleotide substitution at position $-$ 38 reduced P_eps expression threefold, while a doublemutation changing nucleotides at both $-$ 32 and $-$ 29 dramaticallyincreased P_eps expression (Table 2). These data areconsistent with the presumed role of this region as the $-$ 35 consensushexamer that comprises a $sigma$ ⁷⁰-type RNA polymerase recognition site (21).

EpsR can inhibit transcription activation of P_eps by XpsR and VsrC. epsR encodes a putative DNA-binding protein that inhibits EPS production by R. solanacearum strain K60, but only when plasmidborne (18, 25, 30). Moreover, the two reported phenotypesof epsR mutants of strain K60 are contradictory (3, 25).Therefore, we needed to explore a possible role for epsR in regulatingP_eps transcription in our R. solanacearum strain. Todo this we transferred plasmid pKL4 containing the K60 epsR gene(25) into our wild-type AW strain harboring a genomic eps::lacZfusion (AW19A). The addition of pKL4 reduced expression of epsby sevenfold (Table 4). To determine what P_eps sequencesare required for this effect, pKL4 was transferred into strainAW harboring reporter plasmids with different lengths of P_epssequences fused to lacZ (Fig. 1). Expression from reporters withP_eps sequences between $-$ 143 and +23 or between $-$ 101 and+23 fused to lacZ was specifically reduced by greater than ninefoldby the presence of pKL4 (Table 4). However, deletion of P_epssequences between nucleotides $-$ 101 and $-$ 44 eliminated this effect.When pKL4 was placed in a strain harboring fusion plasmid pEPSM9or pEPSM3, which cannot be transcriptionally activated due tomutations in the $-$ 82 to $-$ 62 regulatory region, expression fromP_eps was not significantly decreased. Thus, epsR affectsP_eps only if it has been activated, suggesting that epsRinterferes with transcriptional activation of P_eps mediatedby vsrC and xpsR via the $-$ 82 to $-$ 62 upstream region.

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TABLE 4. Effect of plasmid-borne epsR on expression from wild-type and mutant eps promoters in R. solanacearum

To further investigate P_eps regulation by epsR, we constructed an epsR null mutant of strain AW. Similar to someresults with strain K60 (25), inactivation of epsR did not obviouslyaffect EPS production. Moreover, when genomic (eps130::lacZ) orplasmid-borne (pPSZ20 or pSZ21) P_eps::lacZ fusionswere transferred into the AW strain that lacks EpsR, expressionfrom P_eps was the same as in the wild type (data notshown). Thus, epsR affects P_eps expression in strainAW only when plasmid-borne, probably due to the 10-fold overproductionof EpsR caused by an elevated copy number (25).

Isolation and characterization of vsrB-independent vsrC alleles. Previous genetic studies (19, 20) and analogy to other two-component systems (17) suggest that, in response to somesignal, VsrB phosphorylates VsrC, converting it into a form thatcan activate transcription from P_eps. However, sinceXpsR is also required, this assumption is tentative. To explorethe dependency of VsrC on the VsrB sensor kinase, as well as XpsR,we set out to isolate vsrC alleles that activate P_epsindependently of VsrB and/or XpsR. A pool of 20,000 plasmids containingheavily PCR-mutagenized vsrC alleles was transferred into R. solanacearumstrain AW22B (eps::lacZ vsrB:: $Omega$ ), and transformants with elevatedeps::lacZ expression were selected. After reisolation and retransformationinto AW22B, only one plasmid (pVSRC1) consistently and stronglyincreased P_eps expression in the absence of VsrB. LacZassays showed that in either AW22B or AW22BC (vsrB vsrC eps::lacZ)double mutants, pVSRC1 caused a greater than ninefold increasein transcription of eps::lacZ (Table 5). In contrast, pRKVC3with wild-type vsrC only slightly increased eps expression. Thissuggested that the vsrC1 allele on pVSRC1 harbors a mutation thatmakes it nearly fully active in the absence of phosphorylationby VsrB. When pVSRC1 was placed in the wild-type reporter strainAW22 or strain AW22C (vsrC eps::lacZ), P_eps activationwas similar to that observed in strain AW22BC (Table 5), suggestingthat the activity of VsrC1 cannot be dramatically increased byVsrB. When pVSRC1 was placed in a strain lacking VsrC, VsrB, andXpsR (AW22RBC), transcription of eps::lacZ showed only a small(less than twofold) increase. Restoring vsrB to this strain (i.e.,converting it to a vsrC xpsR mutant) had no effect on its vsrC1-mediatedactivation of P_eps (data not shown). Thus, although VsrC1protein is very active without VsrB, it still requires xpsR forP_eps activation. Not surprisingly, all of our attemptsto isolate vsrC alleles that functioned independently of xpsRby screening the pool of mutant vsrC alleles in xpsR mutants wereunsuccessful.

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TABLE 5. Activation of eps expression by wild-type and mutant alleles of vsrC in various R. solanacearum regulatory mutants

Inactivation of vsrB or vsrC increases PglA production by about sevenfold (19, 20; Fig. 2), indicating that, in additionto positive regulation of eps, the VsrB-VsrC two-component systemnegatively regulates production of polygalacturonase PglA. Placingthe vsrC1 allele in an AW22BC mutant caused its derepressed PglAlevel to be reduced back to wild-type levels (Fig. 2); in contrast,introduction of wild-type vsrC into the same strain did not affectPglA levels. Thus, vsrC1 exhibits both positive and negative regulationof appropriate targets without the input of VsrB.

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FIG. 2. Regulation of pglA by wild-type vsrC and mutant alleles of vsrC. Concentrated supernatants of 24-h-old BSM cultures of strain AW22 (wild-type background [WT]) or from double mutant strain AW22BC (vsrB vsrC) containing the indicated plasmids were serially diluted twofold in BSM and 5 µl of each dilution (2× through 1/8×) spotted on nitrocellulose. The amount of PglA was assayed using anti-PglA antiserum and alkaline phosphatase-conjugated secondary antibody. pRKVC3 contains wild-type vsrC; pVSRC1 and pVSRC2 contain the vsrB-independent alleles vsrC1 and vsrC2, respectively. PglA $-$ , supernatant from R. solanacearum PG3 (pglA::nptl [39]). Purified PglA (50, 25, 12, 6, and 3 µg, respectively, for each of the 5 dilutions listed at the left) was used for calibration.

DNA sequence analysis of the vsrC1 allele showed two nucleotide substitutions: A996 $right-arrow$ G and C1185 $right-arrow$ T, causing substitution ofHis146 with Arg and of Ser 209 with Leu. To explore the contributionof each amino acid substitution to the vsrC1 phenotype, spliceoverlap PCR was used to construct a vsrC allele encoding a VsrCwith only the S209L substitution. When cloned into pRK415 andassayed in regulatory mutants of R. solanacearum, this allele(vsrC2) had essentially the same effect on expression of eps andpglA as the vsrC1 allele (Table 5 and Fig. 2) indicating thatthe vsrB-independent phenotype of vsrC1 and vsrC2 is largely theresult of the S209L substitution. The position of this alteredresidue is unexpected and striking, since the analogous regionin all other response regulators is outside of the helix-turn-helixDNA-binding domain and other regions implicated in their function(17).

In vitro analysis of VsrC binding to P_eps. Genetic data could not distinguish whether VsrC directly binds to and activates P_eps or works via an intermediate,so we investigated the ability of VsrC to bind to P_epsin vitro. First we constructed expression plasmids harboring eitherwild-type vsrC or the constitutively active vsrC1 with their Ntermini translationally fused in frame to a hexahistidine encodingtag. Both His-tagged alleles were nearly as active as wild-typevsrC; when cloned on pRK415 and placed in an R. solanacearum vsrCmutant, both alleles increased eps::lacZ expression by >10-fold,to ca. 50% of wild-type levels (data not shown). After both His-taggedproteins were purified to >90% homogeneity, up to 20 µg of eachwas used in gel mobility shift assays with appropriate ³²P-labeled P_eps fragments. However, no consistent specificmobility shifting was detected under a variety of conditions (datanotshown).

Next we tried a new, rapid footprinting analysis (46) to detect VsrC binding to P_eps. A fragment with the $-$ 337to +23 region of P_eps that was fluorescently labeledat one 5'-end with 6-FAM was briefly incubated with His-VsrC andthen DNase I. Fragmentation patterns were analyzed on an ABI 310Genetic Analyzer. Run outputs, displayed as electropherogramsor "false gel images" (Fig. 3), clearly show an upstream regionof P_eps where the abundance of certain fragments decreaseswith increasing amounts of His-VsrC protein in the reaction. Thisis likely due to a VsrC-specific hindrance of the access of DNaseI to this region (i.e., protection). Supporting this, incubationof the P_eps fragment with a control protein preparationor incubation of purified His-VsrC with a promoter fragment ofa gene not controlled by VsrC did not affect their DNase I fragmentationpatterns (data not shown). We also observed that similar to otherDNA binding proteins, incubation of the P_eps fragmentwith 3 µg of His-VsrC specifically caused increased DNase I cleavage(i.e., hypersensitivity) adjacent to the protected region (Fig.3A). Footprinting reactions using the constitutively active His-VsrC1protein gave essentially the same results (data not shown). Fromthe size of the affected fragments, the positions of nucleotidesspecifically protected (bound) by VsrC were determined to be between $-$ 62 and $-$ 72, the same P_eps region that harbors many nucleotidesimportant for transcription activation by VsrC and XpsR (Table2). The hypersensitive region is upstream between nucleotides $-$ 76 and $-$ 90.

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FIG. 3. DNase I footprinting analysis of VsrC binding to P_eps. Reactions were set up, processed, and analyzed using the ABI 310 as described in Materials and Methods and previously (46). (A) Electropherograms from reactions with increasing amounts of His-VsrC. The y-axis gives fluorescence intensity, which is proportional to fragment abundance; the x-axis gives elution position of fragments, which is proportional to their size. Bottom scale gives nucleotide position relative to the eps transcription start site (21) determined using the elution positions of internal size standards. Solid bar, upstream region of P_eps that is protected from DNase I digestion by His-VsrC. Dashed line, region made hypersensitive by VsrC. The DNA sequence of the protected region, marked with the same bars, is shown above with nucleotides identified by mutagenesis as critical for transcription activation (see Table 2) marked +. (B) "False gel image" representation of electropherograms in panel A generated by Genotyper 2.5 software, which converts the fluorescence intensity of peaks into proportional gray-scale bands. The sequence of the VsrC-protected region is given on the right.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Transcription of eps, an operon encoding biosynthesis of the EPS I virulence factor of R. solanacearum, is controlled by acomplex network composed of at least three interacting and environmentallyresponsive systems (41). We previously found that activationof transcription driven by P_eps sequences downstreamof nucleotide $-$ 143 was completely dependent on xpsR and the vsrB-vsrCtwo-component system (21). Extending that work here, we showedthat sequences downstream of nucleotide $-$ 243 are required andsufficient for wild-type P_eps expression and regulation.However, when P_eps sequences between $-$ 243 and $-$ 143 weredeleted, expression was reduced threefold but remained fully dependenton xpsR and vsrB-vsrC. Thus, the $-$ 243 to $-$ 143 region enhancesthe transcription activation that is mediated by these regulators.The global virulence regulator of R. solanacearum, PhcA (5,41), may play a role in this enhancement, because purified PhcAbinds to and protects the $-$ 185 to $-$ 140 region of P_epsfrom DNase I digestion and because the enhanced activation thatrequires the $-$ 243 to $-$ 143 region is absent in phcA mutants (ourunpublisheddata).

Further promoter deletion experiments clearly showed that nucleotides below $-$ 101 are absolutely critical for activation ofP_eps. Subsequent mutagenesis studies (Table 2) revealedthat many of the critical nucleotides lie between $-$ 82 and $-$ 62,in particular within the GTGGGGAA located between $-$ 74 and $-$ 67.Inactivation of either vsrC or xpsR did not further reduce expressionfrom P_eps fragments with mutations in this region, suggestingthat VsrC and/or XpsR may directly bind to this site to mediatetranscription activation. Using DNase I footprinting we confirmedthat VsrC does indeed directly bind to and protect the $-$ 74 to $-$ 67 region. Recent footprinting experiments (W. Yindeeyoungyeonand M. Schell, unpublished data) have identified another VsrC-protectedbinding site upstream of a new eps gene. The sequences of thesetwo VsrC-protected sites show extensive similarity and suggestthat VsrC may recognize a conserved palindromic consensus sequencefound in both regions (TCCNC-N₈-GGGGA; Fig. 1). However, in contrastto similar footprinting experiments with another DNA-binding protein(46), a >100-fold excess of wild-type or constitutively activeVsrC did not fully protect either site from DNase I, implyingthat the affinity of VsrC for these sites is relatively low. PerhapsXpsR (or another factor) is required for strong binding. In supportof this hypothesis, we found that transcriptional activation byboth wild-type and the constitutively active vsrC1 allele stillrequires xpsR. Although enhancement of DNA binding by an auxiliaryprotein is not a common property of response regulators (17),another R. solanacearum response regulator, VsrD, also requiresan auxiliary protein for its transcriptional regulation (22).Unfortunately, in vitro testing for the effect of XpsR on VsrCbinding has not been possible due to the insolubility of our purifiedXpsR preparation. Alternatively, it is plausible that XpsR maybe involved in the phosphorylation status of VsrC; however, theactivity of VsrC1 in vivo and in vitro was essentially wild typeregardless of the presence of the VsrB sensor kinase. While thesedata suggest that VsrC1 is fully active in the absence of phosphorylation,other possibilities remain. Site-directed mutagenesis of Asp-58in VsrC's receiver domain, the presumed site of phosphorylationby VsrB, should better define the role of VsrB and XpsR in phosphorylationand/or activation of VsrC .

The position of the substitution in VsrC that conferred independence from VsrB (residue 209, 12 residues from the C terminus)is interesting and novel, but not surprising considering thatvsrC1 was the only bona fide VsrB-independent allele found ina population of >20,000 heavily mutagenized alleles. VsrC, a FixJ-typeresponse regulator (17), is very similar to NarL, the crystalstructure of which has been determined (2). Alignment of theC termini of VsrC and NarL (which are 80% similar) suggests thatthe S209L substitution is located in the middle of helix 10 whichfollows the helix-turn-helix DNA-binding domain. The region containinghelix 10 has not been implicated in transcription activation byresponse regulators, nor is its amino acid sequence highly conserved.However, circumstantial evidence that the C terminus of a responseregulator may interact with RNA polymerase has been reported:deletion of the last two or three residues of BvgA severely inhibitedgrowth of Bordetella pertussis, but this effect was suppressedby mutations affecting the $alpha$ -subunit of RNA polymerase (42).We have found that vsrC1 also can cause growth inhibition in R.solanacearum. Since genetic and biochemical evidence suggeststhat interactions between transcriptional regulators and the $alpha$ -subunitof RNA polymerase are sometimes important in transcriptional activation(35), it is plausible that the C-terminal region of some responseregulators (e.g., helix 10) may interact with RNA polymerase tostimulate transcription. Site-directed mutagenesis and chemicalcross-linking studies are required to further investigate thispossibility.

In contrast, most mutations conferring sensor independence on response regulators are N terminal (e.g., V88L for NarL [10]and some N-terminal deletions [13]). These mutations are thoughtto mimic changes caused by sensor kinase-mediated phosphorylation;i.e., they cause a conformational change that alleviates occlusionof the C-terminal helix-turn-helix DNA-binding domain (9, 12).Similarly, the substitution at the C terminus of VsrC1 may alsoalter its conformation in a way that relieves or prevents inhibitoryinteractions of its helix-turn-helix DNA-binding domain with otherparts of the polypeptide that block or reduce itsfunction.

The role of EpsR in P_eps regulation and its relationship to xpsR and vsrC remain unclear, because we found that inactivationof epsR did not dramatically affect expression from P_epsor EPS I biosynthesis, whereas when present on a multicopy plasmid,epsR did reduce P_eps expression by greater than sevenfold.This inhibitory effect occurred only when the VsrC-binding siteat P_eps was intact. Although indirect evidence for thebinding of EpsR to P_eps has been reported (3), wewere unable to confirm this. Preliminary analyses with lacZ reportersshow that elevated levels of EpsR slightly (threefold) reduceexpression of xpsR but not of vsrC. Although this implies thatenvironmentally directed overproduction of EpsR could reduce levelsof XpsR and hence shut down EPS production, further in vivo andin vitro studies are needed to clarify the physiological roleand mechanism of action of EpsR and XpsR with VsrC at the $-$ 82to $-$ 62 region of P_eps.

	ACKNOWLEDGMENTS

This research was supported in part by grant MCB 97-27921 from the National ScienceFoundation.

The authors thank Tim Hoover and Ellen Neidle for critical reading of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, University of Georgia, 527 Biological Sciences Bldg., Athens,GA 30602. Phone: (706) 542-2815. Fax: (706) 542-2674. E-mail:Schell{at}arches.uga.edu.

Present address: Microbiology Department, SmithKline Beecham, Box 5089, Collegeville, PA19436.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ausubel, F., R. Brent, D. Kingston, J. G. Seidman, J. Smith, and K. Struhl. 1996. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.

2. Baikalov, I., I. Schroder, T. Kaczor-Grzeskowiak, K. Grzeskowiak, R. P. Gunsalus, and R. E. Dickerson. 1996. Structure of the Escherichia coli response regulator NarL. Biochemistry 35:11053-11061[CrossRef][Medline].

3. Chapman, M. R., and C. C. Kao. 1998. EpsR modulates production of extracellular polysaccharide in the bacterial wilt pathogen Ralstonia (Pseudomonas) solanacearum. J. Bacteriol. 180:27-34[Abstract/Free Full Text].

4. Clough, S. J., M. A. Schell, and T. P. Denny. 1997. Differential expression of virulence genes and motility in Ralstonia (Pseudomonas) solanacearum during exponential growth. Appl. Environ. Microbiol. 63:844-850[Abstract].

5. Clough, S. J., M. A. Schell, and T. P. Denny. 1997. A two-component system in Ralstonia (Pseudomonas) solanacearum modulates production of PhcA-regulated virulence factors in response to 3-hydroxypalmitic acid methyl ester. J. Bacteriol. 179:3639-3648[Abstract/Free Full Text].

6. Denny, T. P., B. F. Carney, and M. A. Schell. 1990. Inactivation of multiple virulence genes reduces the ability of Pseudomonas solanacearum to cause wilt symptoms. Mol. Plant-Microbe Interact. 3:293-300.

7. Denny, T. P., and S. R. Baek. 1991. Genetic evidence that extracellular polysaccharide is a virulence factor of Pseudomonas solanacearum. Mol. Plant-Microbe Interact. 4:198-206.

8. Denny, T. P. 1995. Involvement of bacterial polysaccharides in plant pathogenesis. Annu. Rev. Phytopathol. 33:173-197.

9. Djordjevic, S., P. N. Goudreau, Q. Xu, A. M. Stock, and A. H. West. 1998. Structural basis for methylesterase CheB regulation by a phosphorylation-activated domain. Proc. Natl. Acad. Sci. USA 95:1381-1386[Abstract/Free Full Text].

10. Egan, S. M., and V. Stewart. 1991. Mutational analysis of nitrate regulatory gene narL in Escherichia coli K-12. J. Bacteriol. 173:4424-4432[Abstract/Free Full Text].

11. Flavier, A. B., S. J. Clough, M. A. Schell, and T. P. Denny. 1998. Identification of $beta$ -hydroxypalmitic acid methyl ester as a novel autoregulator controlling virulence in Ralstonia solanacearum. Mol. Microbiol. 26:251-259.

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13. Gu, B., J. H. Lee, T. R. Hoover, D. Scholl, and B. T. Nixon. 1994. Rhizobium meliloti DCTD, a sigma 54 dependent activator, may be negatively controlled by a subdomain in the C-terminal end of its two-component receiver module. Mol. Microbiol. 13:51-66[CrossRef][Medline].

14. Hanahan, D. 1983. Studies on transformation of Escherichia coli with plasmids. J. Mol. Biol. 166:557-580[Medline].

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19. Huang, J., T. P. Denny, and M. A. Schell. 1993. VsrB, a regulator of virulence genes of Pseudomonas solanacearum, is homologous to sensors of the two-component regulatory family. J. Bacteriol. 175:6169-6178[Abstract/Free Full Text].

20. Huang, J., B. Carney, T. P. Denny, A. K. Weissinger, and M. A. Schell. 1995. A complex network regulates expression of eps and other virulence genes of Pseudomonas solanacearum. J. Bacteriol. 177:1259-1267[Abstract/Free Full Text].

21. Huang, J., and M. A. Schell. 1995. Characterization of the eps gene cluster of Pseudomonas solanacearum and its transcriptional regulation via a single promoter. Mol. Microbiol. 16:977-989[Medline].

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23. Huang, Q., and C. Allen. 1997. Exo-poly- $alpha$ -D-galacturonosidase, PehB, is required for wild-type virulence of Ralstonia solanacearum. J. Bacteriol. 179:7369-7378[Abstract/Free Full Text].

24. Kang, Y., J. Huang, M. Guozhang, L.-Y. He, and M. A. Schell. 1994. Dramatically reduced virulence of mutants of Pseudomonas solanacearum that are defective in export of extracellular proteins across the outer membrane. Mol. Plant-Microbe Interact. 7:370-377.

25. Kao, C. C., F. Gosti, Y. Huang, and L. Sequeira. 1994. Characterization of a negative regulator of exopolysaccharide production by the plant pathogenic bacterium Pseudomonas solanacearum. Mol. Plant-Microbe Interact. 7:121-130[Medline].

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1.	Ausubel, F., R. Brent, D. Kingston, J. G. Seidman, J. Smith, and K. Struhl. 1996. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.
2.	Baikalov, I., I. Schroder, T. Kaczor-Grzeskowiak, K. Grzeskowiak, R. P. Gunsalus, and R. E. Dickerson. 1996. Structure of the Escherichia coli response regulator NarL. Biochemistry 35:11053-11061[CrossRef][Medline].
3.	Chapman, M. R., and C. C. Kao. 1998. EpsR modulates production of extracellular polysaccharide in the bacterial wilt pathogen Ralstonia (Pseudomonas) solanacearum. J. Bacteriol. 180:27-34[Abstract/Free Full Text].
4.	Clough, S. J., M. A. Schell, and T. P. Denny. 1997. Differential expression of virulence genes and motility in Ralstonia (Pseudomonas) solanacearum during exponential growth. Appl. Environ. Microbiol. 63:844-850[Abstract].
5.	Clough, S. J., M. A. Schell, and T. P. Denny. 1997. A two-component system in Ralstonia (Pseudomonas) solanacearum modulates production of PhcA-regulated virulence factors in response to 3-hydroxypalmitic acid methyl ester. J. Bacteriol. 179:3639-3648[Abstract/Free Full Text].
6.	Denny, T. P., B. F. Carney, and M. A. Schell. 1990. Inactivation of multiple virulence genes reduces the ability of Pseudomonas solanacearum to cause wilt symptoms. Mol. Plant-Microbe Interact. 3:293-300.
7.	Denny, T. P., and S. R. Baek. 1991. Genetic evidence that extracellular polysaccharide is a virulence factor of Pseudomonas solanacearum. Mol. Plant-Microbe Interact. 4:198-206.
8.	Denny, T. P. 1995. Involvement of bacterial polysaccharides in plant pathogenesis. Annu. Rev. Phytopathol. 33:173-197.
9.	Djordjevic, S., P. N. Goudreau, Q. Xu, A. M. Stock, and A. H. West. 1998. Structural basis for methylesterase CheB regulation by a phosphorylation-activated domain. Proc. Natl. Acad. Sci. USA 95:1381-1386[Abstract/Free Full Text].
10.	Egan, S. M., and V. Stewart. 1991. Mutational analysis of nitrate regulatory gene narL in Escherichia coli K-12. J. Bacteriol. 173:4424-4432[Abstract/Free Full Text].
11.	Flavier, A. B., S. J. Clough, M. A. Schell, and T. P. Denny. 1998. Identification of $beta$ -hydroxypalmitic acid methyl ester as a novel autoregulator controlling virulence in Ralstonia solanacearum. Mol. Microbiol. 26:251-259.
12.	Goudreau, P. N., and A. M. Stock. 1998. Signal transduction in bacteria: molecular mechanisms of stimulus-response coupling. Curr. Opin. Microbiol. 1:160-169[CrossRef][Medline].
13.	Gu, B., J. H. Lee, T. R. Hoover, D. Scholl, and B. T. Nixon. 1994. Rhizobium meliloti DCTD, a sigma 54 dependent activator, may be negatively controlled by a subdomain in the C-terminal end of its two-component receiver module. Mol. Microbiol. 13:51-66[CrossRef][Medline].
14.	Hanahan, D. 1983. Studies on transformation of Escherichia coli with plasmids. J. Mol. Biol. 166:557-580[Medline].
15.	Hayward, A. C. 1991. Biology and epidemiology of bacterial wilt caused by Pseudomonas solanacearum. Annu. Rev. Phytopathol. 29:65-87.
16.	Hayward, A. C. 1994. Hosts of Pseudomonas solanacearum, p. 9-24. In A. C. Hayward, and G. L. Hartman (ed.), Bacterial wilt: the disease and its causative agent Pseudomonas solanacearum. CAB International, Oxon, United Kingdom.
17.	Hoch, J. A., and T. J. Silhavy. 1995. Two-component signal transduction. ASM Press, Washington, D.C.
18.	Huang, H., and L. Sequeira. 1990. Identification of a locus that regulates multiple functions in Pseudomonas solanacearum. J. Bacteriol. 172:4728-4731[Abstract/Free Full Text].
19.	Huang, J., T. P. Denny, and M. A. Schell. 1993. VsrB, a regulator of virulence genes of Pseudomonas solanacearum, is homologous to sensors of the two-component regulatory family. J. Bacteriol. 175:6169-6178[Abstract/Free Full Text].
20.	Huang, J., B. Carney, T. P. Denny, A. K. Weissinger, and M. A. Schell. 1995. A complex network regulates expression of eps and other virulence genes of Pseudomonas solanacearum. J. Bacteriol. 177:1259-1267[Abstract/Free Full Text].
21.	Huang, J., and M. A. Schell. 1995. Characterization of the eps gene cluster of Pseudomonas solanacearum and its transcriptional regulation via a single promoter. Mol. Microbiol. 16:977-989[Medline].
22.	Huang, J., W. Yindeeyoungyeon, R. P. Garg, T. P. Denny, and M. A. Schell. 1998. Joint transcriptional control of xpsR, the unusual signal integrator of Ralstonia solanacearum virulence gene regulatory network, by a response regulator and a LysR-type transcriptional activator. J. Bacteriol. 180:2736-2743[Abstract/Free Full Text].
23.	Huang, Q., and C. Allen. 1997. Exo-poly- $alpha$ -D-galacturonosidase, PehB, is required for wild-type virulence of Ralstonia solanacearum. J. Bacteriol. 179:7369-7378[Abstract/Free Full Text].
24.	Kang, Y., J. Huang, M. Guozhang, L.-Y. He, and M. A. Schell. 1994. Dramatically reduced virulence of mutants of Pseudomonas solanacearum that are defective in export of extracellular proteins across the outer membrane. Mol. Plant-Microbe Interact. 7:370-377.
25.	Kao, C. C., F. Gosti, Y. Huang, and L. Sequeira. 1994. Characterization of a negative regulator of exopolysaccharide production by the plant pathogenic bacterium Pseudomonas solanacearum. Mol. Plant-Microbe Interact. 7:121-130[Medline].
26.	Keen, N. T., S. Tamaki, D. Kobayashi, and D. Trollinger. 1988. Improved broad-host-range plasmids for DNA cloning in gram-negative bacteria. Gene 70:191-197[CrossRef][Medline].
27.	Kitten, T., and D. K. Willis. 1996. Suppression of a sensor kinase dependent phenotype in Pseudomonas syringae by ribosomal L35 and L20 proteins. J. Bacteriol. 178:1548-1555[Abstract/Free Full Text].
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