Department of Microbiology and Immunology, Health Sciences
Center, West Virginia University, Morgantown, West Virginia
26506-9177,1 Department of Biophysics,
Boston University School of Medicine, Boston, Massachusetts
02118,2 Pfizer Central Research, Groton,
Connecticut 06340,3 and National
Animal Disease Center, United States Department of Agriculture,
Agricultural Research Service, Ames, Iowa 5001014
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INTRODUCTION |
The spirochetes are a
phylogenetically and morphologically unique group of bacteria
(42). This phylum contains not only many medically important
species such as Treponema pallidum and Borrelia
burgdorferi but others that are commensal with arthropods such as
termites and some that are free-living and reside in soil and water
(5, 17, 28, 42). The distinctive spirochete structure has
been characterized in detail. Outermost is a membrane sheath, and
within this sheath is the cell cylinder and periplasmic flagella (PFs).
The PFs reside between the outer membrane sheath and cell cylinder in
the periplasmic space. Each PF is subterminally attached to one end of
the cell cylinder. Several lines of evidence indicate that the PFs are
directly involved in spirochete motility and that these organelles
rotate in a manner similar to that of flagella of other bacteria
(6, 8, 30). The size of the spirochete, the number of PFs
attached at each end of the cell cylinder, and whether the PFs overlap
in the center of the cell vary from species to species (5).
The protein composition of PFs is complex (see 29
for recent review). In contrast to the flagella of most bacterial
species, PFs are comprised of two classes of proteins termed FlaA and
FlaB (3, 8, 39). PFs consist of one to two FlaA proteins and three to four FlaB proteins. B. burgdorferi is an exception,
as this species has one FlaA protein and only one FlaB protein
(11, 14). These proteins share immunological and sequence
similarity within a given class but not between classes. In addition,
these classes show extensive conservation within the spirochete phylum (3, 8, 9, 14, 26, 33, 39, 40, 47, 52). Nucleotide sequence
data and N-terminal amino acid sequence information indicate that FlaA
is likely to be secreted into the periplasmic space via the general
secretory pathway (4, 39, 40, 43). In contrast, FlaB
proteins have significant homology to flagellin of other bacteria in
the N-terminal and C-terminal regions. These proteins are not cleaved
at the N terminus and are most likely secreted into the periplasmic
space by a type-III secretion system (3, 8, 39, 40).
The structure of the spirochete PF is atypical compared to the flagella
of other bacteria. In fact, it is among the most complex of bacterial
flagellar filaments so far studied (8). PFs consist of a
core surrounded by a protein sheath (18, 38, 52). The intact
PF has a diameter of 18 to 25 nm and a core of approximately 11 to 16 nm in diameter (18, 38, 52). Several lines of evidence indicate that FlaA comprises the sheath and that the several FlaB proteins form the core. The evidence includes immunoelectron microscopy of PFs from Spirochaeta aurantia, Leptospira
interrogans, and Brachyspira (formerly
Serpulina, Treponema) hyodysenteriae
(3, 26, 31, 52), partially disrupted cells of T. pallidum analyzed by electron microscopy and Western blot analysis
(9), and analysis of T. pallidum purified PFs by
a Western blotting method termed epitope bridging (2).
The function of the individual PF proteins is poorly understood, as
gene transfer systems have only recently been established for
spirochetes so that specific genes can be inactivated (19, 30, 49,
51). Recently, Rosey et al., using allelic exchange mutagenesis,
inactivated two PF filament genes of the spirochete B. hyodysenteriae, the etiological agent of swine dysentery (44, 45). This spirochete has approximately eight to nine PFs
subterminally attached at each end (5). Based on Western
blot analysis of lysed cells, the PFs were reported to be comprised of
a FlaA protein that migrated as a doublet and three FlaB proteins
designated FlaB1, FlaB2, and FlaB3 (44). The flaA
and flaB1 mutants were found to remain motile but were less
virulent for mice than the wild-type strain, and their swimming
behavior appeared altered (22, 44). In addition, using
electron microscopic analysis of disrupted whole cells revealed that
the diameter of the attached PFs of the flaA mutants were
identical to that of the wild-type strain (44, 45). These
latter results are in conflict with the model that FlaA comprises the
PF sheath. In the work reported here, we constructed the additional
mutants flaB2 and flaB3 and analyzed their
purified PFs and those from the previous mutants in detail. We show
that inactivation of one fla gene specifically inhibited the
incorporation of the encoded protein into the assembled PF. In
addition, we reexamined the PF diameter of the mutants and wild-type
strain and made comparisons. Finally, because little is known about how
each protein influences filament morphology, we examined the PFs of the
wild type and mutants by high-magnification dark-field microscopy. We
show that FlaA influenced the helical shape of the assembled PFs.
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MATERIALS AND METHODS |
Bacterial strains and culture conditions.
Escherichia
coli, Salmonella enterica serovar Typhimurium LT2, and
B. hyodysenteriae B204 and derived mutant strains are listed in Table 1. For convenience, the
flaA1 gene (and its encoded protein) described by Rosey et
al. (44) is referred to as flaA, as no other FlaA
proteins have been detected in both analyses. E. coli and
S. enterica serovar Typhimurium strains were grown in Luria
Bertani medium or 2YT medium (35). B. hyodysenteriae cells were cultured in a Coy chamber using a
premixed gas mixture of 90% N2 with 10% CO2
at 38°C. The equilibrated chamber contained 1 to 2% O2
(measured with a model 3100 oxygen sensor [Biosystems, Inc.,
Middlefield, Conn.]) which is optimal for B. hyodysenteriae (50). B. hyodysenteriae cells were grown in brain
heart infusion broth supplemented with 10% fetal bovine serum
(BHI-FBS) (44). Kanamycin (200 µg/ml) and/or
chloramphenicol (20 µg/ml) were added to the media of appropriate
mutant strains. Mutant strains were cloned by harvesting individual
colonies from Trypticase soy agar plates supplemented with 5% whole
bovine blood (TSAB) instead of the previously used sheep blood
(44).
DNA manipulation and PCR conditions.
Enzyme modification,
subcloning, and transformation were carried out by standard procedures
(35). B. hyodysenteriae chromosomal DNA was
isolated as previously described (44). For amplification of
target genes, the primer sequences, target loci, and binding sites for
target genes are listed in Table 1. DNA amplifications were performed
with Taq (Promega) or VentR polymerases. PCR was carried
out at 95°C for 3 min, followed by 35 cycles of 94°C for 1 min,
52°C for 1 min, 72°C for 2 to 3 min, and a final extension at
72°C for 8 min. The amplified DNA products were purified by using
Qiagen PCR purification kits.
Electrotransformation of B. hyodysenteriae.
The
preparation of competent cells of B. hyodysenteriae and
electroporation were carried out essentially as previously described (44). All manipulations except centrifugations and
electroporations were done in the Coy chamber, and all solutions were
equilibrated at least 12 h in that chamber before use. Briefly, 1 liter of logarithmic-phase cells (5 × 107 to 4 × 108 cells/ml) was chilled on ice for 30 min, harvested
at 9,600 × g for 10 min at 4°C, and resuspended in
100 ml of chilled wash buffer (15% glycerol-272 mM sucrose). After
two washes in this buffer, cells were resuspended in 5 ml. original
volume. The resulting cells (4.5 × 1010 cells/ml)
were maintained on ice until use or stored at 
80°C. Samples were
prepared for electroporation by mixing 90 µl of electrocompetent cells and 1 µg of linearized plasmid DNA or PCR products in 10 µl
in prechilled 0.1-cm cuvettes. Electroporation was carried out using
the Bio-Rad Gene Pulsar II system at 1.5 kV, 25 µF, and 200 
resistance. Such conditions resulted in field strengths of 15 kV/cm
with time constants between 3.8 and 4.5 ms. Following electroporation,
1.5 ml of prewarmed BHI-FBS was immediately added to cuvettes and
transferred to a screw-cap tube (Falcon; 16 by 125 mm) containing a
small stir bar. The recovered cells were incubated in the Coy chamber
overnight with constant stirring. Chloramphenicol was added, and the
cells were cultured for another 18 h. Approximately 0.5-ml samples
were spread onto TSAB plates containing chloramphenicol. Colonies
recovered after 5 to 7 days incubation were inoculated into 3 ml of
BHI-FBS broth containing chloramphenicol.
DNA cloning techniques and screening of the genomic library.
Two degenerative primers were used to clone flaB3. The first
primer was deduced from the variable region near the N-terminal amino
acid sequence obtained by Edman degradation of the gel-extracted purified protein (C. Slaughter, Southwestern Medical School, Dallas, Tex.) (amino acid sequence, TGNSMT [Table 1, primer DFB3]). The second primer, which was directed to a conserved sequence near the
C-terminal region common (amino acid sequence, MIATEN [Table 1 primer
DRB3]) to both FlaB1 and FlaB2 of B. hyodysenteriae, was
obtained using the PepTools alignment program. The 700-bp PCR product
obtained after amplification was cloned into pGEM-T. Double-stranded
DNA sequence analysis, BLAST comparisons with other FlaB proteins, and
comparisons with peptide sequences obtained after trypsin digestion
confirmed that the amplified DNA corresponded to flaB3. To
obtain the entire flaB3 gene, a digoxigenin-labeled 615-bp
PCR probe (random labeling kit [Boehringer Mannheim]) was used to
screen a lambda ZAP II library (Stratagene) of B. hyodysenteriae DNA by standard methods (35). DNA from
plasmids derived from positive plaques were further analyzed using
Southern blotting and DNA sequencing. The GenBank Accession Number for
B. hyodysenteriae flaB3 is AF241832.
Northern blot analysis.
Northern blot analysis was carried
out using standard procedures (35). Approximately 500 ml of
a culture of B. hyodysenteriae was harvested and washed with
cold 0.067 M phosphate-buffered saline (pH 7.5 [PBS]). Total RNA was
isolated and purified using Qiagen RNeasy midikit. The samples were
treated with RNase-free DNase I followed by a clean-up step using
Qiagen RNeasy minikit. RNA samples were run in 1.2% formaldehyde
agarose gels followed by transfer to Hybond-N+ membrane. Targeted genes
were amplified by PCR and were labeled using the North 2South Biotin
Random Prime kit (Pierce), and mRNA was detected using the
Chemiluminescent Nucleic Acid Hybridization and Detection kit (Pierce).
PF purification.
PFs of B. hyodysenteriae were
purified by a method similar to that used to purify PFs from
Treponema denticola (47). One liter of a broth
culture of late-logarithmic-phase cells (approximately 5 × 108 cells/ml) was harvested and centrifuged at
8,000 × g for 8 min at 4°C. The cell pellet was
resuspended and washed twice with cold PBS. Following the second wash,
the cells were resuspended in 90 ml of cold 0.1 M Tris buffer (pH 7.8 [T-buffer]). To remove the spirochete outer membrane sheath, 10 ml of
a 10% (wt/vol) Triton X-100 solution was added dropwise with swirling
and the mixture was incubated for 1 h at 37°C. The lysate was
then centrifuged at 12,000 × g for 20 min at 4°C,
and the pellet containing the PFs and cell cylinders was resuspended in
50 ml of T-buffer. The PFs were sheared from the cell cylinders by
adding 8-ml aliquots to a 50-ml glass tube containing 1-mm glass beads
and were vortexed vigorously for 1 min. After completion, the glass
beads were rinsed with 10 ml of T-buffer, and the pooled mixture was
centrifuged at 18,000 × g for 30 min at 4°C to
remove cellular debris. The supernatant fluid was collected and
centrifuged at 100,000 × g for 1 h at 4°C. The
pellet, consisting of purified PFs, was suspended in either PBS
containing 0.05% sodium azide and stored at 4°C or in T-buffer and
stored at 20°C. Cesium chloride-purified PFs were obtained as
follows: the pellet was suspended in 10 ml of PBS containing 5 g
of cesium chloride and adjusted to a density of 1.270 g/cm2; after centrifugation at 180,000 × g
at 15°C for 4 h, in a Beckman vertical TVi-65.2 rotor, the band
containing the PFs (density, 1.30 g/cm3) was isolated and
centrifuged at 2,000 × g at 4°C in a Centriprep 10 tube (Amicon) to concentrate the PFs; and dialysis in PBS to remove
CsCl followed.
Gel electrophoresis and Western blotting.
Sodium dodecyl
sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) was carried out
as previously reported (14). The resolving gels contained
10% acrylamide and were stained with 0.25% Coomassie blue.
Quantitation of proteins was achieved by using densitometry (Northern
Light Precision Illuminator, model B90, with OPTIMUS 6.2 software
program) on Coomassie blue-stained gels of purified PFs. Ten
determinations were carried out, and each result is expressed as the
mean plus or minus standard error of the mean (SEM). Two-dimensional gel electrophoresis was carried out using a pH range from 3 to 10 ampholytes (Investigator 2-D electrophoresis system) (39, 47). Precast gels were obtained from Genomic Solutions, Ann Arbor, Mich. The second-dimension gel was 10% acrylamide. For Western
blotting, rabbit B. hyodysenteriae polyclonal FlaA and FlaB
antisera were kindly provided by M. Jacques (University of Montreal,
Quebec, Canada) (31). Monoclonal antibody to B. hyodysenteriae FlaB, which reacts with all three FlaB proteins,
was kindly provided by G. Duhamel, University of Nebraska
(10). Antisera directed to T. pallidum FlaA and
to Treponema phagedenis FlaB proteins have been previously
described (32, 33, 39). These latter antisera reacted with
FlaA and FlaB proteins of B. hyodysenteriae, respectively.
We found that the various antisera essentially yielded equivalent
reactions. However, we found that the T. pallidum FlaA antiserum also reacted with FlaB1 of B. hyodysenteriae, and
the T. phagedenis FlaB antiserum sometimes reacted with a
nonflagellar protein of B. hyodysenteriae. Primary
polyclonal antibodies were diluted to 1:5000, and the monoclonal
antibodies were diluted to 1:3 million. Blots were developed by using
horseradish peroxidase-conjugated second antibody with the ECL luminol
assay (Amersham).
Dark-field microscopy.
PF morphology and cell motility were
analyzed using dark-field microscopy (7). Briefly, PFs in
PBS were suspended in approximately equal volumes of 1%
methylcellulose 4000 (Fisher Scientific) also in PBS and observed using
a 100× objective on a Leitz dark-field microscope with a DAGE-MTI
model 72 charge-coupled device (CCD) camera at room temperature. Images
were captured using a Sony Video Graphic printer UP-910. The helix
pitch and helix diameter were measured directly from the video prints
and are expressed as means plus or minus SEM; 25 PFs were measured for
each strain. Significant differences were established using analysis of
variance (ANOVA) and posthoc Tukey-Kramer tests. Flagella isolated from S. enterica serovar Typhimurium strain LT2 served as an
internal control (7).
Both direct observation by microscopy and swarm plate assays were used
to assay for motility. For microscopic assays, cell motility was
determined by harvesting logarithmic-phase cells grown in BHI-FBS in a
microcentrifuge and resuspending the pellet in prereduced PBS or saline
(23). Motility was determined by using dark-field microscopy
both in the presence and absence of 1% methylcellulose
(47). Translational motility was specifically assayed for
each mutant in these medium environments. For swarm plate assays, 4 µl of washed cells suspended in prereduced saline at a density of
approximately 108 cells/ml was spotted on TSAB agar plates
containing 0.3% agarose. After incubation for 36 h at 38°C in
the reduced atmosphere, swarm diameters were determined.
Electron microscopy.
PFs and thin sections were examined by
standard methodology. Approximately 5 µl of the filament suspensions
were placed onto a copper grid (400 mesh) covered with a continuous
carbon foil and blotted after 1 min using Whatman no. 40 filter paper.
Heavy metal staining was performed using a 5-µl drop of 1% uranyl
acetate that was blotted after 15 s. The grids were then allowed
to air dry and were stored in a desiccated, sealed chamber. Images at a
nominal magnification of ×60,000 were recorded onto Kodak SO-163 film
using a Philips CM12 electron microscope operating at an accelerating
voltage of 120 kV. Data were collected at room temperature, and
low-dose techniques were not used. The diameters of the PFs were
measured directly from the photographs using a caliper and are
expressed as means plus or minus SEM. Significant differences were
established using ANOVA and posthoc Tukey-Kramer tests. Not more than
two measurements were made per filament, and at least 12 filaments were
measured per sample. For the preparation of thin sections of B. hyodysenteriae cells, 5 to 10 ml of late-logarithmic-phase cells
were centrifuged at 8,000 × g for 8 min at 4°C.
Cells were fixed, block embedded, and stained as previously described
(15, 30). Sections were viewed with a JEOL 1020 microscope
at an accelerating voltage of 80 kV.
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RESULTS |
Composition of B. hyodysenteriae PFs.
Previous
analyses of B. hyodysenteriae PFs using SDS-PAGE and Western
blot analysis indicated that there were 1 to 2 FlaA proteins and 3 FlaB
proteins (26, 44). In our analysis, we found a single wide
band reacting with the FlaA antiserum (FlaA [44 kDa]) and 3 bands
reacting with the FlaB antiserum (FlaB1 [37 kDa], FlaB2 [34 kDa],
and FlaB3 [32 kDa]) (Fig. 1, lane a). Occasionally, the FlaA band appeared as a doublet by SDS-PAGE and
Western blot. This FlaA doublet has also been observed by Rosey et al.
(44). Proteins with molecular masses of 39, 35, and 29 kDa
were consistently found in the PF preparations (Fig. 1, lane b), but
these proteins failed to react with the FlaA or FlaB antisera. Similar
findings of a 29- to 30-kDa protein in PF preparations have been
reported for PFs of T. pallidum, T. phagedenis,
and T. denticola (39, 47). Because the 39- and the 29-kDa proteins were not detected on CsCl purification of the PFs
(Fig. 1, lane c), these two proteins are likely to be loosely
associated with the PFs. Two-dimensional gel electrophoresis and
Western blot analysis clearly resolved the wide band at 44 kDa into a
smeared doublet (Figure 1, lane d). In contrast to T. phagedenis and T. denticola (39, 47), no
additional major FlaB proteins were resolved with two-dimensional gel
electrophoresis and Western blotting (Figure 1, lane d). The minor spot
to the left of FlaB3 was analyzed in some detail. No differences were detected with this protein compared to FlaB3 by mass spectroscopy of
digested peptides and N-terminal amino acid sequence analysis. In
addition, mutations in the flaB3 gene led to its
disappearance, indicating that the spot was encoded by
flaB3. We consider that this spot is likely an artifact of
two-dimensional gel electrophoresis.
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FIG. 1.
Analysis of wild-type strain B204 periplasmic flagellar
proteins. (a) Western blot analysis of PFs in a single dimension using
B. hyodysenteriae polyclonal FlaA and monoclonal FlaB
antisera. (b) Coomassie blue stain of purified PFs. (c) Coomassie blue
stain of purified PFs after CsCl centrifugation, showing loss of the
39-kDa and 29-kDa proteins. (d) Western blot of a two-dimensional gel
of purified periplasmic flagella, using polyclonal B. hyodysenteriae FlaA and T. phagedenis FlaB antisera.
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Construction of flaB2 and flaB3 allele
replacement vehicles and mutagenesis.
Besides the
flaA::cat,
flaA::kan, and
flaB1::kan mutants already
reported (44), we constructed and also analyzed
flaB2::cat and
flaB3::cat deletion mutants. The
sequence of the flaB2 gene has recently been determined
(25). To target flaB2 for allelic exchange
mutagenesis, it was first amplified by PCR using primers CHB1/CHB2
(Table 1). The product obtained was cloned into pGEM-T to form plasmid
pGFB2 (Fig. 2a). flaB2 was
disrupted by replacement of an internal 345-bp
EcoRI/HindIII fragment with a 922-bp
cat cassette. The insert was flanked with 318-bp upstream
and 246 bp downstream of B. hyodysenteriae DNA. The
orientation of the insert was confirmed by PCR and DNA sequence
analysis, and the resultant linearized plasmid pLNB2 was used for
allelic-exchange mutagenesis.
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FIG. 2.
Construction of plasmids pLNB2 and pLNB3. (a) Plasmid
pGFB2, which contained the intact flaB2 gene, was cut with
EcoRI and HindIII. The resulting 245-bp
deletion was replaced by the purified cat gene from pER187,
yielding pLNB2 (43). (b) Plasmid pGFB3, which contained the
intact flaB3 gene, was cut with EcoRI and
HindIII. The resulting 278-bp deletion was replaced by
the purified cat gene from pER187, yielding pLNB3. The final
linearized plasmids pYNB2 and pYNB3 were used for allelic-exchange
mutagenesis.
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The entire flaB3 gene was cloned and sequenced as described
in Materials and Methods. Using the lambda ZAP II library and a labeled
615-bp flaB3 PCR-amplified product as probe, only one of
several thousand plaques was positive. Sequencing the plasmid insert
revealed an 840-bp open reading frame corresponding to a protein of 280 amino acids and a predicted mass of 30.5 kDa. This predicted size of
FlaB3 approximates the 32-kDa mass estimated from SDS-PAGE analysis
(Fig. 1). After extracting FlaB3 from gels and treating with trypsin,
six internal peptides were sequenced by Edman degradation. The
predicted amino acid sequence deduced from the gene sequence completely
matched that of the obtained FlaB3 peptides (data not shown), thus
confirming that the gene cloned was flaB3.
To construct the flaB3 allelic-exchange vehicle, a 1,185-bp
fragment containing flaB3 and flanking DNA was amplified
using primers CHB5/CHB6 (Table 1). The product obtained was cloned into
pGEM-T to form the recombinant plasmid pGFB3 (Fig. 2b). Cloned flaB3 was disrupted by replacement of an internal 278-bp
EcoRI/HindIII fragment with a 922-bp
cat cassette. The insert was flanked by 621 bp upstream and
286 bp downstream of B. hyodysenteriae DNA. The resultant
flaB3::cat pLNB3 plasmid was further
characterized by PCR analysis and was used for allelic-exchange mutagenesis.
Both of the intact linearized donor plasmids, pLNB2 and pLNB3, were
used to inactivate flaB2 and flaB3 by
allelic-exchange mutagenesis. In addition, PCR products containing the
flaB2::cat and the
flaB3::cat inserts were also successful
in activating flaB2 and flaB3. Following
selection on plates with chloramphenicol, resistant mutants were
screened by PCR with cat primers CAT1/CAT2. Those that were
positive were further tested by PCR with flaB2 primers
CHB3/CHB4 (Fig. 3a) and flaB3
primers CHB7/CHB8 (Fig. 3b). Each of these primers corresponded to
flanking regions outside the input DNA. The
flaB2::cat mutant (A208) yielded a
1,567-bp product rather than the wild-type 990-bp product. The products amplified by CHB3/CAT2 (1,227 bp) and CAT1/CHB4 (1,118 bp) suggested that cat recombined into the chromosomal flaB2
locus. For the flaB3::cat mutant
(A211), the PCR product amplified by CHB7/CHB8 yielded a 1,878-bp
rather than the wild-type 1,234-bp product. The products amplified by
CHB7/CAT2 (1,565 bp) or CAT1/CHB8 (1,234 bp) suggested that
cat was inserted into the chromosomal flaB3 locus. Products amplified by CHB3/CHB4 and CHB7/CHB8 were directly sequenced and were in complete agreement with homologous recombination of the input DNA occurring at flaB2 and flaB3
(data not shown).
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FIG. 3.
PCR analysis of newly constructed flaB
mutants compared with the wild-type strain B204. Ethidium bromide
electrophoresis of DNA-amplified products using primers for analysis of
(a) wild type and flaB2::cat mutant
A208 and (b) flaB3::cat mutant A211 and
wild type. PCR primers are listed in Table 1.
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Mutants assemble PFs without the cognate gene product.
We
analyzed the protein composition of the purified PFs. Previous results
have shown that the deletion mutants
flaA::cat, flaA::kan, and
flaB1::kan had a loss of the
corresponding protein as detected by Western blot analysis of
whole-cell lysates. These mutants still assembled PFs and were motile
(44). Because the protein composition of the purified PFs
was not determined, a mutation in one fla gene could
conceivably have impact on the assembly of the other FlaA and FlaB
proteins in forming the PF. To further analyze the composition and
structure of the PFs of these mutants, along with the newly constructed
flaB2::cat and flaB3::cat mutants, the PFs of the
mutants were purified and compared to the wild type. As with the
previously described flaA::cat, flaA::kan, and
flaB1::kan mutants, the
flaB2::cat and
flaB3::cat mutants were still motile as
determined by dark-field microscopy. Western blot analysis of the PFs
indicated that both flaA::cat and
flaA::kan were deficient in the FlaA
protein found in the wild type (Fig. 4).
In addition, PFs from the flaB1::kan,
flaB2::cat, and
flaB3::cat mutants were specifically
deficient in their respective cognate proteins. A similar pattern was
obtained when whole-cell lysates were probed with the FlaA and FlaB
antisera (data not shown). These results indicated that not only do all
mutants fail to specifically express the mutant gene product but intact
PFs are assembled from the remaining PF proteins. We also determined the ratios of the FlaB proteins relative to FlaA in the wild type and
flaB1::kan and
flaB2::cat mutant in purified PFs. We
found that the wild type had a ratio of FlaB1 to FlaA of 0.42 ± 0.01, of FlaB2 to FlaA of 0.22 ± 0.04, and of FlaB3 to FlaA of
0.45 ± 0.07. In both the
flaB1::kan and
flaB2::cat mutants, these ratios did
not markedly differ from those of the wild type. For example, in the
flaB1::kan mutant, the ratio of FlaB2
to FlaA was 0.34 ± 0.04 and of FlaB3 to FlaA was 0.56 ± 0.04. Similar results were found with the
flaB2::cat mutant (data not shown).
These results suggest that the mutants did not compensate for a given
flaB mutation by producing more of another FlaB protein.
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FIG. 4.
Western blot analysis of purified PFs of mutants and
wild type using B. hyodysenteriae FlaA and FlaB polyclonal
antisera.
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Northern blot analysis.
The analysis of the PF proteins
indicated that a mutation in one gene did not have a polar effect on
the expression of the other flaA and flaB genes.
These results suggested that these genes are not part of an operon. To
further understand the expression of these genes, we analyzed the
transcripts of flaA, flaB1, flaB2, and
flaB3 using Northern blot analysis (Fig.
5). Each of these genes was found to
synthesize a relatively small-sized mRNA of approximately 1 kb. These
results indicated that each of the flagellin genes is transcribed as a
single gene transcript and are consistent with flaB genes
being widely distributed throughout the B. hyodysenteriae strain B78T chromosome as found by Zuerner et al.
(55).
Ultrastructure of the wild-type and mutant PFs.
The PFs of the
wild-type and flaA::cat and
flaA::kan mutants have been reported to
have the same diameter of approximately 15 nm (44, 45).
These results, which were obtained by examining PFs from partially
disrupted cells, are inconsistent with other evidence that FlaA forms a
sheath around the FlaB core. Accordingly, we examined purified PFs of
the wild type and mutants by negative staining and electron microscopy.
The PFs of the wild type consisted of filaments of approximately 25.5 nm in diameter (Fig. 6, left panel).
Occasionally, some PFs were seen that were obviously thinner. In
addition, some appeared thicker at one region and thinner at another
region. These thin PFs and the thin regions on the thicker PFs had
diameters of approximately 18.4 nm. The diameters of the PFs from the
flaB1::kan and
flaB2::cat mutants were similar to that
of the wild type (Fig. 6). In contrast, the diameters of the PFs of the
flaA::cat mutant (19.6 ± 1.8 nm
[Fig. 6, right panel) were significantly thinner than those of the
wild type and flaB1::kan and
flaB2::cat mutants (Fig. 6). In
addition, the flaA::cat mutant PFs were
similar in diameter to the occasional thin PFs seen in the wild type.
Taken together, these genetic results support the immunoelectron
microscopy findings that FlaA forms a sheath around the FlaB core in
B. hyodysenteriae (26, 31). They also support a
similar conclusion reached with other spirochete species PFs (2,
3, 9, 52).
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|
FIG. 6.
Electron microscopic analysis of purified PFs from wild
type and flaA::cat mutant A203. The PF
diameters in nanometers (mean plus or minus SEM) of the wild type and
mutants were as follows: wild type, 25.57 ± 0.23;
flaA::cat, 19.62 ± 0.35;
flaB1::kan, 24.37 ± 0.28;
flaB2::cat, 24.02 ± 0.26;
flaB3::cat, not determined.
flaA::cat was significantly smaller
than the wild type (P < 0.0001).
|
|
Periplasmic flagellar shape.
Bacterial flagella, as well as
PFs from several spirochete species, have been shown to be helical as
determined by high-magnification dark-field microscopy (6, 7,
34). Each spirochete species has been shown to have left-handed
PFs with a distinct helix pitch, helix diameter, and handedness.
Because the PFs consist of multiple proteins, it is not known what role
each protein species plays with respect to overall filament morphology.
Accordingly, we determined the handedness, helix pitch, and helix
diameter of the wild-type and mutant PFs by dark-field microscopy (Fig.
7a through c). We found that the PFs of
the wild-type and mutants were all left handed. The helix pitch of the
wild type was 2.84 ± 0.09 µm with a helix diameter of 0.83 ± 0.04 µm. The PFs from the
flaB1::kan, flaB2::cat, and
flaB3::cat mutants were slightly
smaller in helix pitch and diameter as compared to those of the wild
type. In contrast, the PFs of both
flaA::cat and
flaA::kan mutants had a helix pitch and
helix diameter significantly less than those of the wild type (Tukey's
honestly significant difference (HSD), P < 0.0001).
For example, the flaA::cat mutant A203
had a helix pitch of 2.43 ± 0.15 µm and a helix diameter of
0.61 ± 0.07 µm. These results indicated that mutants deficient
in FlaA have PFs with a markedly altered helical shape.
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FIG. 7.
Analysis of B. hyodysenteriae PF shape. (a)
Dark-field micrographs of purified PFs from wild type and
flaA::cat mutant. (b) Bar graph of
helix pitch and (c) helix diameter of wild type and mutants. Data are
means plus or minus SEM. *, Significance at 0.05 level.
|
|
Number of PFs from wild type and mutants.
The location of the
individual FlaB proteins in a given PF is unknown. A number of possible
structural models have been postulated (44). One model
states that the PFs are heterogenous within a given cell, but
homogeneous with respect to a given filament (44). Thus, for
example, some of the PFs in a given cell could be composed of
FlaAFlaB1, while others could be composed of FlaAFlaB2 and FlaAFlaB3.
If PFs from the mutants were heterogeneous within a given cell, the
flaB1::kan,
flaB2::cat, and
flaB3::cat mutants should have fewer
PFs than the wild type. To test for this possibility, we examined
flaB1::kan and
flaB2::cat mutant cells by thin-section electron microscopy. We found that the number of PFs per cell did not
significantly differ from that of the wild type (Fig. 8). The mean number of PFs varied between
by eight or nine PFs per cell. Because each mutant did not
significantly produce more of the other FlaB proteins to compensate for
its respective mutation (see above), it is unlikely that this number
was achieved by overproducing one of the other FlaB proteins. These
results are not consistent with the proposal that a given PF is
composed of a single FlaB protein in association with FlaA; rather, the
data suggest that a given PF contains FlaA and several different FlaB
proteins (44).
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FIG. 8.
Thin sections of wild type and
flaA::cat and
flaB1::kan mutants.
flaB2::cat was similar (data not
shown), and flaB3::cat was not
determined. The mean numbers of PFs per cell were between 8 and 9 for
the wild type and mutants.
|
|
Motility of wild type and mutants.
Rosey et al.
(44) previously reported that
flaA::cat,
flaA::kan, and
flaB1::kan mutants were motile as
determined by light microscopy, but the behavior of these mutants as
observed by dark-field microscopy appeared different than that of
the wild type. We found that these mutants, along with the newly
obtained flaB2::cat and flaB3::cat mutant strains, could
translate both in PBS and in PBS containing 1% methylcellulose as
observed by dark-field microscopy. Thus, we found that inactivation of
each of the genes which encode the major filament proteins still
results in motile cells. Swarm plate assays were used to quantitatively
assay motility. We found that the swarm diameters of the
flaA::cat,
flaA::kan, and
flaB1::kan mutants were slightly less
than that of the wild type (Fig. 9). These results support those of Rosey et al. that the motility of the
mutants was altered (44). The newly obtained
flaB2::cat and
flaB3::cat mutants also showed smaller
swarms than that of the wild type. Of all the mutants analyzed,
flaB2::cat consistently showed a
smaller swarm diameter than the diameters of the other mutants. These
results indicated that although all the mutants can still assemble PFs,
each appears somewhat deficient in motility, with the
flaB2::cat mutant having the most
deficiency.
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FIG. 9.
Swarm plate assay of wild type and PF mutants. Diameters
of swarms (centimeters) after 36 h of incubation: wild type, 2.1;
flaA::cat, 1.7;
flaB1::kan, 1.7;
flaB2::cat, 1.4;
flaB3::cat, 1.6.
|
|
| |
DISCUSSION |
Spirochetes have historically been a difficult phylum of bacteria
to study. These organisms generally require a rich medium for growth
and have long generation times. Several important spirochete pathogens,
including T. pallidum and many of the oral
Treponema species, have yet to be continuously cultured
(5, 42). Only in B. hyodysenteriae and B. burgdorferi has a gene exchange system been shown to occur by a
mechanism other than via electroporation (19; D. Samuels, personal communication). Compared to the genetic techniques
used to analyze function in other bacteria, the tools now available for
spirochete gene analysis are relatively primitive. The experiments
reported here exploit the use of electroporation and allelic-exchange
mutagenesis as a means to better understand the function of specific PF
genes in B. hyodysenteriae. Because the structure and
composition of the PFs of B. hyodysenteriae (13,
25-27) are so similar to those of T. denticola
(47), L. interrogans (37, 52),
S. aurantia (3, 4, 8, 41), and the more
intractable T. pallidum (39, 40), the results obtained are likely to be relevant to these other species.
Motility is likely to be an important virulence factor for spirochetes
(22, 45, 48). These organisms can swim through gel-like
viscous media, such as connective tissue, which inhibit the motility of
most bacteria (1, 16, 24, 46). B. burgdorferi penetrates the skin after a tick bite, and T. pallidum,
L. interrogans, and B. burgdorferi infect many
tissues of the host, even the eye, which other organisms fail to invade
(20, 24). In addition, genomic analyses of B. burgdorferi and T. pallidum indicate that these
spirochetes have at least 4 to 6% of their genes dedicated to motility
and chemotaxis (11, 12). This relatively large percent of
the genetic material aimed toward these functions reinforces the role
of motility and chemotaxis in the survival of these bacteria within the
hosts that they parasitize and in which, in some cases, they cause
disease. For B. hyodysenteriae, mutants which have altered
PFs and motility also are less virulent in mice, which again reinforces
the role of motility for certain species of spirochetes (22,
45).
In our analysis of the PF proteins of B. hyodysenteriae, we
found that two-dimensional gel electrophoresis enhanced resolution of
the FlaA PF proteins, but no new FlaB proteins were detected. FlaA
appeared as a smeared doublet of approximately 43 to 44 kDa. Our
results are similar to those of Rosey et al., who found a FlaA doublet
of approximately the same molecular masses (44). One of the
proteins in the doublet is likely to be a precursor to the other rather
than each being encoded by a separate gene. Specifically, inactivation
of flaA inhibits synthesis of both proteins in the doublet.
Because Northern blot analysis indicates that flaA is
synthesized as a monocistronic mRNA, it is unlikely that the results
obtained are related to a polar effect on gene expression. The broad
band observed for FlaA may be related to post-translational
modification. Along these lines, Li et al found that FlaA is likely to
be glycosylated (31). Glycosylated proteins often appear
smeared in two-dimensional gel electrophoresis. Our results differ from
those of Koopman et al., who found two FlaA proteins with masses of 44 and 35 kDa (26). One possible explanation for this
difference may be related to the strains tested; we used strain B204 as
did Rosey et al. (44), whereas Koopman used strain C5
(26).
Our results, in conjunction with the previous results of Rosey et al.
(44), indicate that mutants with single mutations in
flaB1, flaB2, or flaB3 were still
motile and could synthesize PFs. Moreover, based on the parameters
measured, the morphology of the PFs was not markedly altered in the
flaB mutants. Alignment of the deduced amino acid sequences
of the three FlaB proteins shows between 37 and 51% identity, with the
N-terminal region most conserved (data not shown). These findings,
coupled with the mutational analysis, indicate that the FlaB proteins
are at least somewhat redundant with respect to function. These results are analogous to flagella formation in Caulobacter,
Helicobacter, and Campylobacter spp. Each of
these species synthesizes multiple flagellin filament species, and
inactivation of one of the encoding genes still results in the
retention of motility and filament synthesis, although in each species
the motility of the mutants is altered (21, 36, 54).
FlaA impacts the shape of the PFs as determined by measuring the helix
pitch and helix diameter of the purified PFs. Because the helix pitch
and diameter of the PFs of the
flaA::cat and
flaA::kan mutants were markedly less
than those of the wild type, evidently the presence of FlaA results in
an increase in helicity. It may be that the sheath structure per se
influences the overall shape of the PFs. Along these lines, preliminary
evidence with a double flaB mutant and with a
fliG mutant indicate that the sheath can form a hollow tube
independently of the core in B. hyodysenteriae (C. Li and
N. W. Charon, unpublished data). Because bacterial flagella are
often quasirigid and undergo helical transformations (34,
53), perhaps the sheath helps stabilize the FlaB helical core
into one of these configurations for optimal thrust as it rotates
between the outer membrane sheath and cell cylinder. We anticipate that
future genetic experiments will allow us to determine the nature of the
interaction of FlaA with the multiple FlaB proteins and how these
proteins participate in achieving optimal cell motility.
We thank S. Humphrey, R. Macnab, and especially D. Yelton for
helpful discussions; X. M. Gao for help in the construction of
pLNB2; J. D. Ruby for help on periplasmic flagella purification methodolgy, G. Hobbs for help with statistics, S. Dodson for help in
cloning flaB3, and D. Berry for assistance with electron
microscopy. We also thank G. Duhamel, M. Jacques, and S. Norris for
antisera, and R. Yancey for encouragement.
This research was supported by Public Health Service grant DE12046, and
by USDA grant 95-37204-2132.
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Abstract
Introduction
