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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.
Department of Microbiology1 and Department of Plant Pathology,2 University of Georgia, Athens, Georgia 30602-2604
Received 18 May 2000/Accepted 6 September 2000
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ABSTRACT |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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High-level transcription of eps, an operon encoding
biosynthesis of an exopolysaccharide virulence factor of the
phytopathogen Ralstonia (Pseudomonas)
solanacearum, requires the products of at least seven
regulatory genes (phcA, phcB, xpsR,
vsrA-vsrD, and vsrB-vsrC), which are organized
in three converging signal transduction cascades. Because
xpsR and the vsrB-vsrC two-component system are
the most downstream cascade components required for activation of
eps, we explored how these components control transcription from the eps promoter (Peps).
Deletion and PCR mutagenesis identified an upstream region of
Peps (nucleotides 
82 to 62) that is
critical for transcription activation by VsrB-VsrC and XpsR and also is
required for negative control of Peps by the
putative eps regulator EpsR. Using PCR mutagenesis we
generated the vsrC1 allele that encodes a response
regulator that constitutively activates Peps in
the absence of its cognate sensor, VsrB. However, activation of
Peps by vsrC1 still required xpsR. Unexpectedly, the amino acid substitution conferring
the constitutive 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 demonstrate specific
binding of both VsrC1 and VsrC to the 72 to 62 upstream region of
Peps.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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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 roots and then proceeds to extensively colonize xylem vessels of the vascular system (37, 44). Although secreted plant cell wall-degrading exoenzymes enhance virulence (possibly by facilitating invasion and vascular colonization [23, 24, 37]), it is exopolysaccharide I (EPS I), a large, nitrogen-rich, acidic exopolysaccharide (34), that is the primary virulence factor of R. solanacearum. EPS I is produced in copious amounts and is required for wilting and killing of hosts (8, 29). EPS I apparently causes wilting by restricting water flow through xylem vessels (6). It also markedly 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 more than 10 regulatory genes (5, 11, 20, 41). Inactivation of any of seven genes in this network causes a >85% reduction in transcription from the eps promoter (Peps), leading to loss of EPS I production and the ability to wilt and kill. However, inactivation of all but two of these genes (vsrB and vsrC) can be suppressed by constitutive expression of xpsR from a vector promoter (20). These and other data showed that VsrB, VsrC, and XpsR are the most downstream components in the eps regulatory cascade and suggested that they may directly affect interaction of RNA polymerase with Peps.
The predicted amino acid sequences of VsrB and VsrC imply that they comprise a two-component system in which VsrB is a sensor kinase and VsrC is its cognate response regulator (19, 20). However, no homologs of the very basic XpsR protein have been found. How these three proteins interact to control Peps is not clear. Nonetheless, analogy to other two-component systems (17) implies that, in response to some unknown signal, VsrB phosphorylates VsrC, thereby stimulating it to turn on transcription, possibly via direct binding to Peps. EpsR, a putative DNA-binding protein, is another potential regulator of Peps, since its overproduction strongly represses EPS I synthesis by R. solanacearum strain K60 (18, 25).
Since there was no clear or direct evidence for physical interactions between Peps and VsrC, XpsR, or EpsR, we first used deletion and PCR mutagenesis to define an upstream region of Peps that is absolutely required for its transcription activation by VsrB-VsrC and XpsR. Then we generated a vsrC allele that activated Peps independently of vsrB and used DNase I footprinting to show that both this constitutively active VsrC protein and wild-type VsrC directly bind to the region of Peps that was identified by mutagenesis to be important in transcription activation. However, since the affinity of VsrC for Peps was weak and since the constitutively active VsrC protein was unresponsive to VsrB and still required XpsR for activation of Peps, we speculate that XpsR may facilitate or stabilize binding of VsrC to Peps.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Bacteria and plasmids.
Most strains and plasmids constructed
and used in this work are described in Table
1. R. solanacearum was grown
in BG or BSM medium (36) at 30°C, while Escherichia
coli was grown in LB (33) at 37°C. The host strain
and vectors used for cloning were E. coli DH5
(14) and pTZ19U/18U (31), respectively. pPF12
(7) and pEPS1 (21) were described previously.
R. solanacearum strain 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 used to select and maintain
plasmids were kanamycin (Km), 50; spectinomycin (Sp), 50; ampicillin
(Amp), 100; and tetracycline (Tc), 20.
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Construction of Peps reporter
plasmids.
Peps 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 denaturation at 94°C for 1 min,
annealing at 50°C for 1 min, and extension at 72°C for 1 min. After
30 cycles, there was a final extension at 72°C for 10 min. The
Peps DNA fragments from nucleotides 538 to
+23, 337 to +23, and 243 to +23 were amplified using pXPS1 as
template and primer pairs EPS6-EPS4, EPS7-EPS4, and EPS9-EPS4, respectively. The Peps DNA fragments from 143
to +23, 101 to +23, 68 to +23, and 44 to +23 were amplified using
primer pairs M13F-EPS4, EPS1-EPS4, EPS2-EPS4, and EPS3-EPS4,
respectively, and pXPS5 as template. PCR products were digested with
BamHI and/or SmaI and ligated into the
promoterless lacZ fusion vector pRG970 (43)
digested in the same manner. After transformation into E. coli and plating on LB agar with Sp and
5-bromo-4-chloro-3-indolyl-
-D-galactopyranoside (X-Gal),
plasmid DNA was isolated from blue colonies, and the orientation and
identity of the insert were confirmed.
PCR mutagenesis of Peps and
vsrC.
To mutagenize Peps, sequences
between nucleotides 143 and +23 were PCR amplified essentially as
above using a pTZSZ12 template. However, the dATP concentration was 0.2 mM instead of 1 mM, and MnCl2 was added to 0.5 mM.
BamHI-digested PCR products were ligated with
BamHI-digested pRG970 and transformed into E. coli, and ~10,000 blue-colored transformants arising on LB
plates with Sp and X-Gal were individually picked and pooled, and
plasmid DNA was isolated from them. Pooled plasmids were electroporated into R. solanacearum strain AW201
(epsA1::nptl). After plating on 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, transformed into E. coli, reisolated, and analyzed with restriction enzymes to confirm
Peps inserts. Sequence alterations were
determined after recloning inserts into pTZ19U.
eps::lacZ). After selection on BG
plates with X-Gal and Tc, transformants showing increased expression of
the eps::lacZ reporter (i.e.,
darker-blue color) were analyzed.
To construct the vsrC2 allele, vsrC sequences
between nucleotides 523 and 1,194 (GenBank U18134) were amplified using
a pRKVC3 template, a T7 primer, and a primer containing vsrC
sequences between nucleotides 1,162 and 1,194 but having a C1185T
mutation (S209L) and a same-sense C1171G silent mutation that
introduced a BamHI site
(5'-TCCATGCGCAAGATGATCTGGATCCGCGTGCGC-3'). The resultant PCR
product and a plasmid with sequences 1,145 to 1,290 of vsrC were mixed, and PCR amplification was performed with T7 and M13F primers. The 800-bp vsrC PCR product was digested with
HindIII and EcoRI and cloned into pRK415.
Plasmids from transformants were isolated and screened for the
introduced BamHI site. The vsrC allele from one
candidate plasmid (pVSRC2) was sequenced to confirm that it contained
the S209L mutation.
Purification of His-tagged VsrC proteins. Wild-type vsrC was PCR amplified using pKVC3 as template and primers M13F and VSRCN (5'-ACGGATCCACGAGCTCGCTGCG-3'; complementary to sequences encoding the N terminus of VsrC). The product was digested with BamHI and cloned in frame to the hexahistidine-encoding tag of BamHI-digested pTrc-HisA (Invitrogen), yielding plasmid pVSRCH. To generate pCB92, the SacI-KpnI fragment of pVSRCH was replaced with the analogous fragment from pVSRC1.
E. coli JM109 (45) cells containing pVSRCH or pCB92 were shaken at 37°C in LB plus Amp until the optical density at 600 nm (OD600) was 0.6. The 100-ml culture was shifted to 28°C, and isopropyl--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 times for 10 s. The sonicate was centrifuged at
30,000 × g for 25 min, and the supernatant was passed
through a 3-ml column containing 1 ml of Ni-nitriloacetic acid resin
(Sigma) equilibrated with buffer B. The column was washed with 10 ml of
buffer B followed by 10 ml of buffer B with 50 mM imidazole. VsrCs were
eluted with buffer B plus 0.5 M imidazole; sodium dodecyl
sulfate-polyacrylamide gel 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 extension were at 70°C. Primers (EPSRN, 5'-AAGGATCCAGG CGGCGCAGTG-3' [nucleotides 355 through 381 with an added BamHI site] and EPSRC, 5'-ATGAATTCAGCCCGGCGTGCACGAGGCG-3' [nucleotides 1,055 through 1,075 with an added EcoRI site]) were based on the sequence of epsR from R. solanacearum strain K60 (GenBank M61197). The resultant PCR product was digested with BamHI and EcoRI and cloned into pTZ18U. DNA sequencing showed that epsR from strain AW is >97% identical to epsR from strain K60.
To construct the epsR null mutant, an internal StyI fragment lacking sequences encoding the first 12 N-terminal residues and last 52 C-terminal residues of EpsR was made blunt ended with T4 DNA polymerase and then cloned into the SmaI site of suicide vector pTOK2 (27). The resultant plasmid (pEPSR-T) was electroporated into R. solanacearum AW, and strains in which the plasmid integrated into epsR by a single recombination event were selected by Tc resistance. Genomic DNA from two strains was prepared and disruption of the genomic copy of epsR was confirmed by PCR; no PCR products could be obtained using EPSRN and EPSRC primers, whereas a PCR product of the predicted size was obtained with wild-type DNA as template. An EPSRN and M13R vector primer gave a PCR fragment of the size predicted for the truncated epsR gene.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 mM Tris HCl [pH 7.4], 140 mM NaCl), the membrane was washed three times with TBST (TBS with 0.2% Tween 20) and submerged for 1 h in 10 ml of TBST containing a 1:1,000 dilution of anti-PglA antiserum (39). After three washes with TBST, one with TBST containing 0.85 M NaCl, and one with TBST, bound PglA antibodies were detected with anti-rabbit immunoglobulin G (IgG) conjugated to alkaline phosphatase (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, pPSZ17 as template, and primers *M13L
(5'-[6-FAM]-CACGACGTTGTAAAACGACGGCCAGT-3'; PE Applied
Biosystems) and T7. The resultant PCR product (containing sequences
between 337 and +23 of Peps and labeled at one
5' end with the 6-FAM fluorescent tag) was gel purified, and 40 ng (10 nM) was used in 10-µl footprinting-reaction mixtures that 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-tagged VsrC proteins. The
total protein concentration was maintained at 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-free DNase I (1.2 × 10
5
U/µl, freshly diluted [Boehringer Mannheim]) were added. After 4 min, 15 µl of 0.5 M EDTA (pH 8.0) was added; reactions were extracted
with phenol-chloroform and passed through a CENTRI-SEP column
(Princeton Separations). Digestion products were vacuum dried,
dissolved in 12 µl of deionized formamide, 0.2 µl of GS-500-ROX size standards (PE Biosystems) was added, and the fragmentation patterns were analyzed with an ABI 310 Genetic Analyzer as described previously (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-treated competent cells or into R. solanacearum via electroporation were described earlier (21, 22). Restriction enzymes, DNA ligase, Klenow fragment, and other DNA enzymes were used according to the manufacturer's recommendations. DNA sequences were obtained using an ABI 377 sequencer. Other general molecular genetic techniques used are described elsewhere (1, 28).
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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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
Peps, we constructed a series of reporter
plasmids with various lengths of Peps fused to
lacZ. Expression of these reporter genes was assayed in an
R. solanacearum wild-type strain and in strains lacking key
regulators. A reporter plasmid with sequences between 538 and +23 of
Peps fused to lacZ(pPSZ15) gave a
high level of Peps expression that was strongly
dependent on both xpsR and vsrC, since
Peps expression was reduced at least 50-fold by
inactivation of either regulator (Fig.
1). Deletion of sequences upstream of
337 or 243 did not dramatically alter expression or regulation,
indicating that sequences between 243 and +23 are sufficient for
wild-type expression from Peps. When sequences
between 243 and 143 were deleted (pPSZ12 [Fig. 1]), expression
was reduced about threefold, suggesting that a site in the region
between nucleotides 243 and 143 stimulates Peps expression. Residual expression from this
reporter construct, however, remained strongly dependent on both
vsrC and xpsR. Deletion of sequences between
143 and 101 did not significantly reduce transcription below that
observed with a reporter having the 143 to +23 region of
Peps fused to lacZ. However, when
sequences between nucleotides 101 and 68 were deleted, Peps expression was reduced to less than 5% of
the levels observed with the 243 to +23 fusion. Expression was only
marginally further reduced when Peps sequences
down to 44 were deleted (pPSZ22 [Fig. 1]), regardless of the
genetic background. These data show that the 101 to 68 region
contains sequences that are absolutely required for activation of
Peps by these two regulators.
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Determination of nucleotides required for activation and regulation
of Peps.
To delineate more precisely the
sequences that are critical for Peps regulation,
a fragment with Peps nucleotides 143 to +23
was subjected to mutagenic PCR, and the products were joined to
lacZ on pRG970 to generate transcriptional fusions. The
resultant pooled reporter constructs were introduced into wild-type
R. solanacearum, and colonies were screened for altered Peps::lacZ expression by
using X-Gal. Sixteen mutant plasmids were obtained and characterized
further by DNA sequencing and quantitative LacZ assays (Table
2).
Peps::lacZ expression from
plasmids with single-nucleotide substitutions at
Peps nucleotides 74, 71, 70, and 69 was
reduced ~10-fold, almost to the basal levels given by plasmids in
which all upstream activation sequences had been deleted (compare to pPSZ22 and pPSZ21 [Fig. 1]). When assayed in xpsR or
vsrC mutants of R. solanacearum, expression
directed by these mutant promoters was only marginally reduced,
indicating that these mutations largely eliminate activation of
Peps transcription by VsrC and XpsR. Fusion
plasmids with single nucleotide substitutions at Peps nucleotides 82, 79, 72, 68, and
67 were reduced about fivefold. However, when assayed in
xpsR or vsrC mutant backgrounds of R. solanacearum, Peps expression from these
promoters was reduced an additional three- to fourfold to basal levels, indicating that these mutant promoters are inefficiently activated by
VsrC and XpsR. In summary, these results suggest that nucleotides between 82 and 62, and in particular the sequence GTGGGGAA
between 74 and 67 (Fig. 1), are important for activation of
Peps. It is plausible that this region contains
the binding sites for Peps activators, perhaps
VsrC and/or XpsR.
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538
and 143 were restored in the proper orientation and position to the Peps::lacZ fusion plasmids
with substitutions at 67 or 72 and the resultant plasmids placed in
wild-type R. solanacearum, Peps
expression was largely the same as observed with shorter (143 to +23)
Peps fragments (Table 2 versus Table
3). These results support the conclusion
that the primary Peps regulatory sequences
required for transcription activation by VsrC and XpsR lie downstream
of nucleotide 143, while sequences upstream of 143 can only enhance
activation by these regulators.
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12, 9,
and 7) also dramatically reduced Peps
expression (Table 2). The position and nature of these mutations are
consistent with the presumed role of this region as the 10 consensus
hexamer of the promoter (21). A single-nucleotide
substitution at position 38 reduced Peps
expression threefold, while a double mutation changing nucleotides at
both 32 and 29 dramatically increased Peps
expression (Table 2). These data are consistent with the presumed role
of this region as the 35 consensus hexamer that comprises a
70-type RNA polymerase recognition site (21).
EpsR can inhibit transcription activation of
Peps by XpsR and VsrC.
epsR encodes
a putative DNA-binding protein that inhibits EPS production by R. solanacearum strain K60, but only when plasmid borne (18, 25,
30). Moreover, the two reported phenotypes of epsR
mutants of strain K60 are contradictory (3, 25). Therefore,
we needed to explore a possible role for epsR in regulating Peps transcription in our R. solanacearum strain. To do this we transferred plasmid pKL4
containing the K60 epsR gene (25) into our
wild-type AW strain harboring a genomic
eps::lacZ fusion (AW19A). The addition
of pKL4 reduced expression of eps by sevenfold (Table
4). To determine what
Peps sequences are required for this effect,
pKL4 was transferred into strain AW harboring reporter plasmids with
different lengths of Peps sequences fused to
lacZ (Fig. 1). Expression from reporters with Peps sequences between 143 and +23 or between
101 and +23 fused to lacZ was specifically reduced by
greater than ninefold by the presence of pKL4 (Table 4). However,
deletion of Peps sequences between nucleotides
101 and 44 eliminated this effect. When pKL4 was placed in a strain
harboring fusion plasmid pEPSM9 or pEPSM3, which cannot be
transcriptionally activated due to mutations in the 82 to 62
regulatory region, expression from Peps was not
significantly decreased. Thus, epsR affects Peps only if it has been activated, suggesting
that epsR interferes with transcriptional activation of
Peps mediated by vsrC and
xpsR via the 82 to 62 upstream region.
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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 some signal, VsrB phosphorylates VsrC,
converting it into a form that can activate transcription from
Peps. However, since XpsR is also required, this
assumption is tentative. To explore the dependency of VsrC on the VsrB
sensor kinase, as well as XpsR, we set out to isolate vsrC
alleles that activate Peps independently of VsrB
and/or XpsR. A pool of 20,000 plasmids containing heavily
PCR-mutagenized vsrC alleles was transferred into R. solanacearum strain AW22B (eps::lacZ
vsrB::), and transformants with elevated eps::lacZ expression were selected.
After reisolation and retransformation into AW22B, only one plasmid
(pVSRC1) consistently and strongly increased
Peps expression in the absence of VsrB. LacZ assays showed that in either AW22B or AW22BC (vsrB vsrC
eps::lacZ) double mutants, pVSRC1 caused a
greater than ninefold increase in transcription of
eps::lacZ (Table
5). In contrast, pRKVC3 with wild-type
vsrC only slightly increased eps expression. This suggested that the vsrC1 allele on pVSRC1 harbors a mutation
that makes it nearly fully active in the absence of phosphorylation by
VsrB. When pVSRC1 was placed in the wild-type reporter strain AW22 or
strain AW22C (vsrC eps::lacZ),
Peps activation was similar to that observed in
strain AW22BC (Table 5), suggesting that the activity of VsrC1 cannot
be dramatically increased by VsrB. When pVSRC1 was placed in a strain
lacking VsrC, VsrB, and XpsR (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-mediated activation of Peps
(data not shown). Thus, although VsrC1 protein is very active without
VsrB, it still requires xpsR for Peps
activation. Not surprisingly, all of our attempts to isolate
vsrC alleles that functioned independently of
xpsR by screening the pool of mutant vsrC alleles
in xpsR mutants were unsuccessful.
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G and C1185T, causing substitution
of His146 with Arg and of Ser 209 with Leu. To explore the contribution of each amino acid substitution to the vsrC1 phenotype,
splice overlap PCR was used to construct a vsrC allele
encoding a VsrC with only the S209L substitution. When cloned into
pRK415 and assayed in regulatory mutants of R. solanacearum,
this allele (vsrC2) had essentially the same effect on
expression of eps and pglA as the
vsrC1 allele (Table 5 and Fig. 2) indicating that the
vsrB-independent phenotype of vsrC1 and
vsrC2 is largely the result of the S209L substitution. The
position of this altered residue is unexpected and striking, since the
analogous region in all other response regulators is outside of the
helix-turn-helix DNA-binding domain and other regions implicated in
their function (17).
In vitro analysis of VsrC binding to Peps. Genetic data could not distinguish whether VsrC directly binds to and activates Peps or works via an intermediate, so we investigated the ability of VsrC to bind to Peps in vitro. First we constructed expression plasmids harboring either wild-type vsrC or the constitutively active vsrC1 with their N termini translationally fused in frame to a hexahistidine encoding tag. Both His-tagged alleles were nearly as active as wild-type vsrC; when cloned on pRK415 and placed in an R. solanacearum vsrC mutant, both alleles increased eps::lacZ expression by >10-fold, to ca. 50% of wild-type levels (data not shown). After both His-tagged proteins were purified to >90% homogeneity, up to 20 µg of each was used in gel mobility shift assays with appropriate 32P-labeled Peps fragments. However, no consistent specific mobility shifting was detected under a variety of conditions (data not shown).
Next we tried a new, rapid footprinting analysis (46) to detect VsrC binding to Peps. A fragment with the337 to +23 region of Peps that was
fluorescently labeled at one 5'-end with 6-FAM was briefly incubated
with His-VsrC and then DNase I. Fragmentation patterns were analyzed on
an ABI 310 Genetic Analyzer. Run outputs, displayed as
electropherograms or "false gel images" (Fig.
3), clearly show an upstream region of
Peps where the abundance of certain fragments
decreases with increasing amounts of His-VsrC protein in the reaction.
This is likely due to a VsrC-specific hindrance of the access of DNase I to this region (i.e., protection). Supporting this, incubation of the
Peps fragment with a control protein preparation or incubation of purified His-VsrC with a promoter fragment of a gene
not controlled by VsrC did not affect their DNase I fragmentation patterns (data not shown). We also observed that similar to other DNA
binding proteins, incubation of the Peps
fragment with 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-VsrC1 protein gave essentially the same results (data not shown).
From the size of the affected fragments, the positions of nucleotides specifically protected (bound) by VsrC were determined to be between 62 and 72, the same Peps region that harbors
many nucleotides important for transcription activation by VsrC and
XpsR (Table 2). The hypersensitive region is upstream between
nucleotides 76 and 90.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Transcription of eps, an operon encoding biosynthesis
of the EPS I virulence factor of R. solanacearum, is
controlled by a complex network composed of at least three interacting
and environmentally responsive systems (41). We previously
found that activation of transcription driven by
Peps sequences downstream of nucleotide 143
was completely dependent on xpsR and the
vsrB-vsrC two-component system (21). Extending
that work here, we showed that sequences downstream of nucleotide 243
are required and sufficient for wild-type Peps
expression and regulation. However, when Peps
sequences between 243 and 143 were deleted, expression was reduced
threefold but remained fully dependent on xpsR and
vsrB-vsrC. Thus, the 243 to 143 region enhances the
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 PhcA binds to and protects the 185 to 140 region of
Peps from DNase I digestion and because the
enhanced activation that requires the 243 to 143 region is absent
in phcA mutants (our unpublished data).
Further promoter deletion experiments clearly showed that nucleotides
below 101 are absolutely critical for activation of Peps. Subsequent mutagenesis studies (Table 2)
revealed that 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 expression from Peps
fragments with mutations in this region, suggesting that VsrC and/or
XpsR may directly bind to this site to mediate transcription
activation. Using DNase I footprinting we confirmed that VsrC does
indeed directly bind to and protect the 74 to 67 region. Recent
footprinting experiments (W. Yindeeyoungyeon and M. Schell, unpublished
data) have identified another VsrC-protected binding site upstream of a
new eps gene. The sequences of these two VsrC-protected
sites show extensive similarity and suggest that VsrC may recognize a
conserved palindromic consensus sequence found in both regions
(TCCNC-N8-GGGGA; Fig. 1). However, in contrast to similar
footprinting experiments with another DNA-binding protein (46), a >100-fold excess of wild-type or constitutively
active VsrC did not fully protect either site from DNase I, implying that the affinity of VsrC for these sites is relatively low. Perhaps XpsR (or another factor) is required for strong binding. In support of
this hypothesis, we found that transcriptional activation by both
wild-type and the constitutively active vsrC1 allele still requires xpsR. Although enhancement of DNA binding by an
auxiliary protein is not a common property of response regulators
(17), another R. solanacearum response regulator,
VsrD, also requires an auxiliary protein for its transcriptional
regulation (22). Unfortunately, in vitro testing for the
effect of XpsR on VsrC binding has not been possible due to the
insolubility of our purified XpsR preparation. Alternatively, it is
plausible that XpsR may be involved in the phosphorylation status of
VsrC; however, the activity of VsrC1 in vivo and in vitro was
essentially wild type regardless of the presence of the VsrB sensor
kinase. While these data suggest that VsrC1 is fully active in the
absence of phosphorylation, other possibilities remain. Site-directed
mutagenesis of Asp-58 in VsrC's receiver domain, the presumed site of
phosphorylation by VsrB, should better define the role of VsrB and XpsR
in phosphorylation and/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 that vsrC1 was the
only bona fide VsrB-independent allele found in a population of
>20,000 heavily mutagenized alleles. VsrC, a FixJ-type response
regulator (17), is very similar to NarL, the crystal structure of which has been determined (2). Alignment of the C termini of VsrC and NarL (which are 80% similar) suggests that the
S209L substitution is located in the middle of helix 10 which follows
the helix-turn-helix DNA-binding domain. The region containing helix 10 has not been implicated in transcription activation by response
regulators, nor is its amino acid sequence highly conserved. However,
circumstantial evidence that the C terminus of a response regulator may
interact with RNA polymerase has been reported: deletion of the last
two or three residues of BvgA severely inhibited growth of
Bordetella pertussis, but this effect was suppressed by
mutations affecting the -subunit of RNA polymerase (42). We have found that vsrC1 also can cause growth inhibition in
R. solanacearum. Since genetic and biochemical evidence
suggests that interactions between transcriptional regulators and the
-subunit of RNA polymerase are sometimes important in
transcriptional activation (35), it is plausible that the
C-terminal region of some response regulators (e.g., helix 10) may
interact with RNA polymerase to stimulate transcription. Site-directed
mutagenesis and chemical cross-linking studies are required to further
investigate this possibility.
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 thought to mimic changes caused by sensor kinase-mediated phosphorylation; i.e., they cause a conformational change that alleviates occlusion of the C-terminal helix-turn-helix DNA-binding domain (9, 12). Similarly, the substitution at the C terminus of VsrC1 may also alter its conformation in a way that relieves or prevents inhibitory interactions of its helix-turn-helix DNA-binding domain with other parts of the polypeptide that block or reduce its function.
The role of EpsR in Peps regulation and its
relationship to xpsR and vsrC remain unclear,
because we found that inactivation of epsR did not
dramatically affect expression from Peps or EPS
I biosynthesis, whereas when present on a multicopy plasmid, epsR did reduce Peps expression by
greater than sevenfold. This inhibitory effect occurred only when the
VsrC-binding site at Peps was intact. Although
indirect evidence for the binding of EpsR to
Peps has been reported (3), we were
unable to confirm this. Preliminary analyses with lacZ
reporters show that elevated levels of EpsR slightly (threefold) reduce expression of xpsR but not of vsrC. Although this
implies that environmentally directed overproduction of EpsR could
reduce levels of XpsR and hence shut down EPS production, further in
vivo and in vitro studies are needed to clarify the physiological role and mechanism of action of EpsR and XpsR with VsrC at the 82 to 62
region of Peps.
| |
ACKNOWLEDGMENTS |
|---|
This research was supported in part by grant MCB 97-27921 from the National Science Foundation.
The authors thank Tim Hoover and Ellen Neidle for critical reading of the manuscript.
| |
FOOTNOTES |
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* 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, PA 19436.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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