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Infection and Immunity, March 1999, p. 1393-1404, Vol. 67, No. 3
Department of Microbiology and Molecular
Genetics1 and Shipley Institute of
Medicine,2 Harvard Medical School,
Boston, Massachusetts 02115
Received 6 October 1998/Returned for modification 18 November
1998/Accepted 10 December 1998
The Vibrio cholerae genome contains a 5.4-kb
pil gene cluster that resembles the Aeromonas
hydrophila tap gene cluster and other type IV-A pilus assembly
operons. The region consists of five complete open reading frames
designated pilABCD and yacE, based on the
nomenclature of related genes from Pseudomonas aeruginosa and Escherichia coli K-12. This cluster is present in both
classical and El Tor biotypes, and the pilA and
pilD genes are 100% conserved. The pilA gene
encodes a putative type IV pilus subunit. However, deletion of
pilA had no effect on either colonization of infant mice or
adherence to HEp-2 cells, demonstrating that pilA does not
encode the primary subunit of a pilus essential for these processes.
The pilD gene product is similar to other type IV prepilin peptidases, proteins that process type IV signal sequences. Mutational analysis of the pilD gene showed that pilD is
essential for secretion of cholera toxin and hemagglutinin-protease,
mannose-sensitive hemagglutination (MSHA), production of
toxin-coregulated pili, and colonization of infant mice. Defects in
these functions are likely due to the lack of processing of N termini
of four Eps secretion proteins, four proteins of the MSHA cluster, and
TcpB, all of which contain type IV-A leader sequences. Some
pilD mutants also showed reduced adherence to HEp-2 cells,
but this defect could not be complemented in trans,
indicating that the defect may not be directly due to a loss of
pilD. Taken together, these data demonstrate the
effectiveness of the V. cholerae genome project for
rapid identification and characterization of potential virulence factors.
Vibrio cholerae is
a gram-negative bacterial pathogen that causes the waterborne
diarrheal disease cholera. Following ingestion by a host and entry
into the upper intestine, V. cholerae colonizes the
intestinal mucosa and begins to export enterotoxins, including the
major virulence toxin, cholera toxin (CT). The activity of CT elicits
severe diarrhea in the infected host, resulting in extreme dehydration,
the hallmark of cholera.
Although extensive research has elucidated the key features of toxin
production and regulation, the basic mechanism underlying the initial
colonization of the intestine by V. cholerae remains elusive. Much work to date has focused on the identification of V. cholerae pili. V. cholerae produces
at least three morphologically distinct types of pili (17).
The first type, the toxin-coregulated pili (TCP), are bundle-forming
pili that are coordinately regulated with CT (53). These
pili are absolutely essential for colonization of the intestine by
V. cholerae, both in the infant mouse colonization model and in human volunteers (2, 20, 40, 50, 53, 55). However, several observations suggest that TCP may not be directly required for adherence. Purified TCP do not bind to human intestinal epithelium, and the adherence of V. cholerae to
intestinal epithelium and various epithelial cell lines is not
blocked by growth under non-TCP-inducing conditions or by anti-TCP
antibodies (3, 12, 48, 51). Further, when classical
V. cholerae strains are grown under
TCP-expressing conditions, the bacteria aggregate, suggesting that TCP
plays a key role in bacterium-to-bacterium adhesion (9, 53).
These observations indicate that other V. cholerae
factors may mediate cellular adherence.
A second type of V. cholerae pili, mannose-sensitive
hemagglutination (MSHA) pili, has also been investigated. These
investigations have been done almost exclusively with El Tor
strains because classical strains produce few or no pili
(26). Within the El Tor strains, MSHA pili are essential for
the hemagglutination of erythrocytes, although no other role in
adherence or pathogenesis has been ascribed to these pili (24,
25). Disruption of the gene encoding the primary pilin subunit,
mshA, has no effect on colonization of infant mice (2,
55) or on disease symptoms in human volunteers (50).
Further, spontaneous mutants defective in hemagglutinating activity
adhere well to intestinal tissue samples (42, 54). Recently,
it was shown that MSHA pili mediate the adherence of V. cholerae El Tor strains to solid substrates, suggesting that they
are important for survival in the environment rather than in the host
(58).
Interestingly, the major pilin subunits of both TCP and
MSHA pili, TcpA and MshA, respectively, are members of the type IV protein superfamily (25, 46). The type IV proteins all
have recognizable N-terminal leader sequences that specify
cleavage and N-methylation by specific prepilin leader peptidases
(21). In addition to MshA and TcpA, V. cholerae contains at least eight other type IV proteins: EpsG,
EpsH, EpsI, and EpsJ, which are part of a type II export machinery that
secretes CT and other toxins; MshB, MshC, and MshD, which are part of
the MSHA pilus assembly machinery; and TcpB, a protein essential for
the production of TCP (25, 31, 40, 44). The tcpJ
gene encodes a prepilin peptidase that processes TcpA into a form that
can be assembled into TCP. Surprisingly, the disruption of
tcpJ abolishes TCP assembly but does not affect either toxin
secretion or hemagglutination of erythrocytes (28). This
result suggests that a second prepilin peptidase is responsible for
processing of the Eps and Msh proteins (28). The
identification of a third type of pili by electron microscopy studies
also suggests that another, uncharacterized pilus may be present in
V. cholerae (17).
Recent progress by The Institute for Genomic Research
(Gaithersburg, Md.) on the V. cholerae genome
project has facilitated the rapid identification of genes of particular
interest. In this paper, we describe the use of early data releases to
identify a new gene cluster that is similar to type IV-A pilus assembly gene clusters. Proteins encoded by this gene cluster include a second
prepilin peptidase that is important for toxin secretion, MSHA, and TCP
production, as well as a new, putative type IV pilin protein. However,
a role in pathogenesis for this pilin protein could not be established.
Bacterial strains and growth conditions.
The V. cholerae strains used in this study are listed in Table
1. Escherichia coli DH5
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Genetic Characterization of a New Type IV-A Pilus Gene
Cluster Found in Both Classical and El Tor Biotypes of
Vibrio cholerae
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
and
DH5
pir were used for construction of plasmids. SM10pir and
2115 were used to deliver plasmids to V. cholerae by
conjugation. All strains were grown on Luria-Bertani (LB) medium at
37°C, except as noted otherwise. Antibiotics (micrograms per
milliliter) used were as follows: ampicillin, 50; chloramphenicol, 4;
kanamycin, 50; and streptomycin, 100.
TABLE 1.
V. cholerae strains used in
this studya
PCR and DNA sequencing.
All oligonucleotides used for PCR
and DNA sequencing were obtained from Biosynthesis, Inc. (Lewisville,
Tex.) or Operon Technologies (Alameda, Calif.) and are listed in Table
2. PCR was performed with TaKaRa
Taq polymerase and reagents from Oncor (Gaithersburg, Md.),
PCR Supermix from Gibco BRL (Gaithersburg, Md.), or Vent Taq
polymerase and reagents from New England BioLabs (Beverly, Mass.). PCR
templates were prepared by suspending a single bacterial colony in 200 µl of distilled H2O, of which 1 µl was used in either a
25- or a 50-µl PCR amplification. For sequencing of the
pil operon and for preparation of all plasmids,
colonies of V. cholerae N16961 or N16961Sm were used as
the PCR template, except as noted otherwise. All PCRs were performed
with standard amplification parameters and an MJ Research Thermocycler
(model PTC-200). For direct sequencing, PCR products were purified by
two passages over a QiaQuick PCR purification kit (Qiagen, Valencia,
Calif.). Automated DNA sequencing was done at the Harvard Microbiology Core Sequencing Facility. The reported sequence has a minimum of
fourfold coverage with at least two sequences for both the coding and
the noncoding strands. The DNA sequence was assembled and open reading
frames were assigned with the GeneWorks Analysis software package.
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Construction of counterselectable plasmids.
pKJF306 is a
streptomycin-based counterselectable plasmid which generates kanamycin
insertions in pilD. Primers PILD1 and PILD2 were used in a
Taq polymerase PCR to generate a 908-bp product encompassing
the pilD gene; this fragment was ligated directly into the
TA cloning vector pCR2.1 (Invitrogen, Carlsbad, Calif.) to create
pKJF302. The fragment was then moved to pBluescript IIKS(+)
(Stratagene, La Jolla, Calif.) as an EcoRI fragment to generate pKJF303. The kanamycin resistance cassette kan
(Pharmacia, Piscataway, N.J.) as an HaeIII fragment and inserted into
pilD on pKJF303 between two Eco47III sites found
at nucleotides (nt) 294 and 334 of the pilD PCR product to
generate pKJF305. The entire pilD::kan fragment
was then moved into the streptomycin-based counterselectable plasmid
pKAS32 (47) as an EcoRI fragment, generating
plasmid pKJF306.
Construction of pilD-complementing plasmids. Primers PILD1 and PILD2 are designed to introduce EcoRI and SalI sites at the 5' and 3' ends of pilD, respectively. Following PCR amplification, the 908-bp product was treated for 20 min at 72°C with Taq polymerase to add an adenosine nucleotide to the termini for direct cloning into pCR2.1 to create pKJF304. The novel EcoRI and SalI sites were then used to move pilD into the pBAD18 (15) polylinker, placing pilD under the control of the arabinose-inducible promoter PBAD but with its own ribosome binding site. For alternative antibiotic selection, the pilD insert was moved from pBAD18 to pBAD18Cm (15) by use of a unique MluI site found on both plasmids and SalI from the polylinker. The resulting plasmids, pKJF308 and pKJF308Cm, were transferred to V. cholerae by electroporation.
Generation of mutations in V. cholerae strains
by use of counterselectable markers.
Counterselectable plasmids
pKJF306 (pKAS32 pilD::kan), pKJF313 (pKAS46
pilA), pKJF324 (pWM91 pilD), pKJF329 (pWM91
pilA), pDLT (pCVD442 lacZ
[57a]), pHT1 (pCVD442 mshA1
[55]), pHT3 (pCVD442 tcpA10
[55]), and pCVDHapSal (pCVD442 hapA
[17a]) were introduced into V. cholerae by conjugation on an LB agar plate. Counterselections
were done by the protocol of Metcalf et al. (34). Briefly,
four cointegrants were purified by streaking one time under selection
and then were passaged one time without selection to allow
recombination to occur. Sixteen independent colonies were then streaked
on the counterselection medium: LB medium containing streptomycin
at 3 mg/ml for streptomycin-based selection and LB medium without
NaCl but containing 6% sucrose for sucrose-based selection. Best
results were achieved when counterselection plates were incubated at
room temperature for 2 days. Isolated colonies were checked by PCR for
gain of the mutation and loss of the wild-type gene.
Agg and CTX
transduction.
Classical V. cholerae cultures were grown in 5 ml of LB broth at 30°C with
rolling for optimal production of TCP (11). The autoagglutination (Agg) phenotype was scored visually. For CTX transductions, phage were prepared by filtering culture supernatant of
Peru-15(CTX-Km) or O395(CTX704A) with a 0.2-µm-pore-size syringe filter. Fifty microliters of phage preparation was mixed with
50 µl of TCP-expressing culture, and the mixture was allowed to
stand for 45 min at room temperature to allow for infection by the
phage and expression of antibiotic resistance genes. The mixture was
then diluted and plated. The transduction frequency is expressed as the
CFU of transductants over the CFU of the recipient strain.
CT assay. For optimal toxin production, classical strains and El Tor strains containing plasmid pBAD18Cm-ToxT (19) were grown at 30°C with rolling for 16 h. One milliliter of culture was spun down in a microcentrifuge, and the culture supernatant was set aside. The bacterial cells were resuspended in 1 ml of 10 mM Tris-HCl-1 mM EDTA-20% glucose (pH 7.5) and sonicated (Branson Sonifier 350) twice for 15 s each time on 20% power. CT present in 100 µl of culture supernatant or sonicate was measured by the GM1-ganglioside enzyme-linked immunosorbent assay with purified CT to generate a standard curve (11).
HAP assays. The presence of hemagglutinin-protease (HAP) was detected on LB agar plates containing 1% nonfat milk (37). For some assays, 4 ml of agar was solidified in divided glass plates such that different quadrants contained different antibiotics and/or inducing compounds.
MSHA assays. MSHA assays were performed as previously described, except that washed defibrinated sheep blood was substituted for human or chicken erythrocytes (12).
Infant mouse colonization.
Overnight cultures of
V. cholerae strains were diluted 1:100 in fresh LB
medium and grown with rolling to the mid-log to late log phase.
Cultures were diluted in 0.15 M NaCl, and 8 µl of blue food coloring
was added. Five- to 7-day-old infant mice were taken from their mothers
at least 5 h prior to oral infection. Fifty microliters of
inoculum was delivered orally to anesthetized mice. Mice were kept at
30°C for a full 24 h, at which time they were sacrificed and
their intestines were dissected from above the cecum. The intestines
were homogenized in 5 ml of LB broth, diluted, and plated on LB agar
with streptomycin and
5-bromo-4-chloro-3-indolyl--D-galactopyranoside (X-Gal). For competition assays, CFU of blue (mutant) and white (wild-type) strains were counted, and the colonization index was calculated as the ratio of blue colonies to white colonies.
HEp-2 cell adherence assays. Overnight cultures of V. cholerae strains were diluted 1:100 in fresh LB medium and grown at 37°C with rolling to the mid- to late-log phase. Bacterial cells were washed in phosphate-buffered saline (PBS) and adjusted to 109 bacteria per ml. Ten microliters was added to HEp-2 epithelial cells (ATCC F-13959) that had been grown in RPMI 1640 medium containing 10% fetal calf serum without antibiotics in 24-well dishes to 105 cells per well. For classical strains, plates were spun for 10 min at 300 × g and incubated at 37°C in 5% CO2 for 1 h. Cells were washed four times with PBS, and adherent bacteria were recovered in 1 ml of PBS-0.1% Triton X-100. For El Tor strains, plates were spun for 2 min and incubated for 15 min to reduce nonspecific adherence to the plastic. Cells were washed and recovered in 1 ml of PBS-1.0% Triton X-100. Percent adherence was calculated as CFU adherent divided by CFU added times 100.
Nucleotide sequence accession number. The nucleotide sequence reported in this study was assigned GenBank accession no. AF109904.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Bioinformatics and sequencing of the pil gene cluster of V. cholerae. The publicly available sequences from the V. cholerae genome project (56a) were examined for the presence of open reading frames with known functions in pathogenesis. Interestingly, sequence runs GVCCS46F and GVCCS46R contain sequences with similarity to two genes found in type IV-A pilus assembly operons (Fig. 1). In addition, sequence runs GVCCP66R and GVCCY88R encode a novel type IV cleavable pilin protein that is closely related to the type IV-A pilin subunit of Pseudomonas aeruginosa (Fig. 1). In order to show that sequences GVCCP66R and GVCCS46F are linked on the V. cholerae genome, primers PILA1 and PILC1 were used in a PCR to amplify a 2.6-kb product representing the intervening region. Primers PILD1 and PILD2 were used to generate a 908-bp product to demonstrate the linkage of GVCCS46F and GVCCS46R (data not shown). The entire 5,401-bp gene cluster was sequenced directly from progressively smaller PCR products such that the operon was sequenced with a minimum of fourfold coverage with at least two sequences for each strand. All sequences from the original data release by The Institute for Genomic Research were also confirmed by the same method.
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The V. cholerae pil gene cluster resembles other type IV-A pilus gene clusters. The 5,401-bp region of V. cholerae contains five complete open reading frames, apparently organized into a single operon. The designation vcpD has been proposed for the fourth gene of this cluster (32), based on the nomenclature of the V. vulnificus operon (38). However, the name vvpA, appropriate for the first gene by this nomenclature, has already been used to describe a V. vulnificus protease gene (6). To avoid further confusion, the nomenclature for P. aeruginosa, the organism with the first identified type IV pilus operon, has been adopted for the first four open reading frames, pilABCD, and the fifth gene is referred to as yacE, consistent with the E. coli genome project designation. As a whole, the cluster is referred to as the pil gene cluster.
The organization of the V. cholerae pil gene cluster shows a striking similarity to that of the Aeromonas hydrophila tap gene cluster (Fig. 1). Although other organisms also tend to group these five genes, V. cholerae and A. hydrophila are apparently the only organisms which group these genes into a single operon. Presumably, the V. vulnificus operon is similarly arranged, although only vvpC, vvpD, and yacE have been identified to date. Interestingly, like the type IV-A pilus assembly operon from E. coli, the V. cholerae pil gene cluster is linked to ampD and nadC, demonstrating that the arrangement of these genes is well conserved between these two gram-negative species. The first open reading frame, pilA, has two potential translation start sites. The second start site was selected because a consensus ribosome binding site is located just upstream of the AUG, whereas no such site is present upstream of the first potential start site. Further, consistent with the grouping of V. cholerae PilA into the type IV-A family, the use of the second translation start site would give a type IV signal sequence of 11 amino acids. Use of the first potential translation start site would give PilA a long signal sequence of 25 amino acids, a feature more common in type IV-B pilin subunits, such as V. cholerae TcpA (13). Although the amino acid sequence similarity among the type IV-A pilins is generally localized to the first 30 amino acids, the sequence of the pilA gene from classical strain O395 is 100% identical at both the protein and the nucleotide levels to the El Tor strain N16961 gene sequence, indicating that the pilA gene is highly conserved in V. cholerae. The next two open reading frames, pilB and pilC, are likely to encode proteins essential for the assembly of a new type IV pilus (1). Recent work with P. aeruginosa has shown that pilB and pilC are merely 2 of up to 30 genes essential for the assembly of type IV pili. These genes include pilT, pilE, and pilU (1), for which open reading frames are also present in the V. cholerae genome (56a). The fourth open reading frame encodes a putative member of the type IV prepilin peptidase family. These proteins recognize the type IV signal sequence and cleave the signal at a conserved glycine (36). The peptidase then modifies the next residue to the form that is assembled into either pili or other membrane structures (49). Like the pilA gene, the V. cholerae pilD gene is 100% conserved between the classical strain O395 and the El Tor strain N16961Sm. The fifth open reading frame, yacE, is a member of a family of genes whose localization with type IV pilus assembly gene clusters is frequently conserved (Fig. 1), although its function is unknown.Effect of various pilD mutations on growth
patterns.
To test whether pilD encodes a prepilin
peptidase essential for secretion and hemagglutination, we constructed
a pilD mutant in which the kanamycin resistance cassette,
kan, was inserted into the pilD gene by double homologous
recombination with the streptomycin-based counterselectable plasmid
pKJF306. Following mating into O395 and N16961Sm, cointegrants were
counterselected on streptomycin and kanamycin to select for loss of the
integrated plasmid and for maintenance of the kan cassette. However,
following the selection process, only pinpoint colonies were recovered
for both O395 and N16961Sm parental strains. These slowly growing mutants, designated KFV5 and KFV18 (Fig.
2), respectively, reverted to a faster
growth pattern with a high frequency when grown in liquid cultures.
Revertants for these strains were single colony purified and designated
KFV5R and KFV18R, respectively.
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insertion were not successful. However, it has been
reported that slowly growing pilD mutants of N. gonorrhoeae can revert to faster growth by accumulating deletions
in the pilin subunit gene, pilE (10). In
accordance with this result, a nonpolar deletion of the pilD gene could be constructed in a pilA deletion background.
However, as shown in Fig. 3B, this mutant, designated KFV36, grew more slowly than the wild type. Also, deletion of pilA from the
classical deletion mutant KFV32 did not enhance its growth beyond that
shown in Fig. 3A (data not shown). Thus, it seems that, in the absence of pilD, PilA precursor proteins are not processed and
contribute in part, but not entirely, to slow growth.
V. cholerae pilD is essential for the secretion of CT and HAP. The eps operon of V. cholerae encodes a type II secretion system that is essential for the export of CT, HAP, and other V. cholerae toxins (37, 44). Four of the proteins encoded by this operon, EpsG, EpsH, EpsI, and EpsJ, contain type IV signal sequences, although a gene for a type IV peptidase is absent from this operon (44). The signal sequence of EpsG is cleaved by N. gonorrhoeae PilD but not by V. cholerae TcpJ (44). These observations suggest that the newly recognized pilD gene of V. cholerae may encode a prepilin peptidase essential for toxin secretion.
To determine if pilD of V. cholerae is essential for the processing of EpsG, EpsH, EpsI, and EpsJ, the various pilD mutants were analyzed for defects in the secretion of CT and HAP. As shown in Fig. 4A, wild-type classical strain O395 exported 97% of the CT that it produced. In contrast, most of the CT produced by mutants KFV5R and KFV32 accumulated within the bacteria and was not exported (Fig. 4A). Export could be restored by the introduction of pilD on a plasmid under the control of the arabinose-inducible promoter PBAD. The export of CT was not complemented either by the pBAD18 vector alone or in the absence of the inducer arabinose (data not shown).
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pilA
pilD double mutant KFV36 (data not shown), although the
small-colony phenotype of this strain alone could account for this
defect, since HAP expression is proposed to be regulated by quorum
sensing (22).
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El Tor pilD mutants are defective in MSHA. El Tor strains of V. cholerae produce a pilus that can hemagglutinate erythrocytes, but not in the presence of mannose (24). The major subunit of this pilus, MshA, and three accessory pilus assembly proteins, MshB, MshC, and MshD, have type IV cleavable sequences although, similar to the situation with the eps operon, a type IV prepilin peptidase is not encoded by the msh gene cluster (18, 25, 32). If pilD is essential for the construction of the MSHA pilus, then pilD mutants should be unable to hemagglutinate erythrocytes.
N16961Sm hemagglutinated sheep erythrocytes, and this hemagglutination was inhibited by both mannose and the nonhydrolyzable analog methyl--D-mannopyranoside but not by fucose or arabinose (Table 3). A deletion within the
mshA gene in N16961Sm abolished this hemagglutination.
Similarly, the El Tor pilD mutants KFV18R and KFV36 did not
hemagglutinate erythrocytes. Hemagglutination was restored when these
strains were complemented with pKJF308, which carries pilD
in trans, but not when they carried the pBAD18 vector or
were grown without arabinose to induce the expression of
pilD on the plasmid (Table 3).
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pilD mutants do not produce wild-type levels of TCP. TCP are type IV pili of the B subfamily, members of which typically have longer type IV signal sequences than type IV-A pili and are carried on mobile elements, such as plasmids or pathogenicity islands (13). Since TcpJ processes the major TCP pilin subunit TcpA (28), it is not expected that pilD mutants should be defective for TCP production. However, it is possible that the essential accessory protein, TcpB (40), is processed by PilD. If this is the case, pilD mutants should be defective for TCP production.
When classical strain cultures are grown under conditions which favor TCP production (11), wild-type strain O395 aggregates, and this aggregation is dependent upon the presence of TCP, since mutants with mutations in tcpA, tcpB, and other tcp genes failed to aggregate (40) (Table 4). Similarly, pilD mutants KFV5R and KFV32 failed to aggregate in cultures, demonstrating a general defect in TCP assembly due to mutation of pilD.
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-Km (kanamycin resistance) and CTX704A (ampicillin
resistance), filamentous transducing phages which adsorb to TCP during
the infection process (57). Wild-type strain O395 was
transduced by both phages at a frequency of 10
2, but
tcpA and tcpB mutants could not be transduced
(Table 4). pilD mutants KFV5R and KFV32 showed an
intermediate phenotype. Although phage transduction was not
completely abolished, pilD mutants KFV5R and KFV32 were
transduced at a 150- to 240-fold-lower frequency (Table 4).
Surprisingly, CTX transduction not only was restored but also was
slightly enhanced by the presence of pilD in
trans.
These data indicate that pilD is very important, although
not absolutely essential, for TCP production. We thus propose that TcpA
is processed primarily by TcpJ (28), while TcpB is processed primarily by PilD, although residual processing by TcpJ may occur. Further, the overproduction of TCP when the copy number of
pilD is increased suggests that the processing of TcpB by
PilD may be a limiting factor in TCP production.
pilD mutants do not colonize infant mice.
Since
TCP production is absolutely essential for colonization,
pilD mutants should not colonize infant mice. Indeed,
strains KFV5R and KFV32 did not colonize infant mice when inoculated
either by themselves or in competition with a lacZ
derivative of O395 (Table 5).
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insertion in pilD and continued to be
defective for HAP export and MSHA, indicating that they did not arise
from in vivo selection for reversion or suppression of the original
pilD mutations. Further, these mouse-recovered KFV18R
isolates did not have enhanced infection capability when inoculated
into new infant mice (data not shown). These observations demonstrate
that while KFV18R fails to colonize well, the mutant is able to
survive the in vivo environment. These observations support the notion
that the loss of colonization is due either to the loss of TCP alone or
to the loss of another pilD-processed protein as well.
pilA and mshA are not required for the
colonization of infant mice.
If the loss of an additional
pilD-processed protein contributes to the colonization
defect, it is possible that the defect is due to pilA, which
is linked to pilD. However, mutants with deletions of
pilA, in both the classical and the El Tor backgrounds, colonized mice as well as the wild type (Table
6). Similarly, mutants with mutations in
the MSHA pilus colonized infant mice as well as the wild type (2,
55) (Table 6). We considered that PilA and MshA might have
redundant functions in colonization. However, double pilA
mshA mutants also colonized mice as well as the wild type
(Table 6). Since CT itself may play an important role in colonization
(41), its presence might mask other adherence factors.
However, pilA mutants of toxin-deficient strains O395N1 and
P4 also showed no defect in colonization compared to the wild type
(Table 6). Thus, we conclude that while pilA may encode a
pilin protein for a new type IV pilus, this putative pilus is not
required for colonization in the infant mouse model.
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Classical pilD mutants adhere poorly to HEp-2 cells due to mutation of an unknown gene. Given that PilD proteins in other organisms process proteins required for epithelial cell adherence (7, 16, 27, 38, 43), we examined the ability of V. cholerae mutants to adhere to HEp-2 cells to determine whether potential adherence factors other than TCP are absent in pilD mutants. When grown under conditions optimal for adherence, O395 adheres to HEp-2 cells. In contrast, the pilD mutant KFV5R adhered poorly compared to the wild type, showing up to a 10-fold defect in repeated assays (Fig. 6A). Surprisingly, unlike other pilD-dependent processes, this defect could not be restored by pilD in trans (Fig. 6B). This result shows that the loss of adherence is most likely due to a gene or protein that was terminally mutated during reversion of the pilD mutation. Unfortunately, attempts to demonstrate an adherence defect in deletion strain KFV32 could not be interpreted because wild-type strains grown to a low density also failed to adhere (data not shown).
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The adherence of El Tor strains to HEp-2 cells is not
pilD dependent.
Determining the adherence of N16961Sm
derivatives proved to be difficult, compared to that for the classical
strains. We recently showed that V. cholerae El Tor and
O139 strains produced a toxin that caused rounding and detachment of
HEp-2 cells (30). The destruction of cellular integrity due
to this toxin hampered interpretation of the results. Further, it
was recently shown that MSHA pili mediated adherence to solid
substrates, including laboratory plastic and glass items used for
tissue culturing (58). To circumvent these technical
difficulties, KFV18R with a disruption of the cytotoxin was compared to
KFV11 (mshA), which also had a disruption of the
cytotoxin. Both strains showed 3% adherence to HEp-2 cells. This
result shows that the loss of pilD and the subsequent
reversion of growth defects to generate KFV18R did not permanently
disrupt a key adhesin. However, the level of adherence was quite low
compared to that observed for classical strains, suggesting that
conditions favoring adherence by El Tor strains may be different from
those for classical strains.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In recent years, the new field of functional genomics has expanded for prokaryotic research. It has been predicted that most of the important human bacterial pathogens will be completely sequenced by the year 2000 (52). The new challenge presented to researchers concerns the use of this plethora of information in designing and performing informative experiments. While sequencing of the V. cholerae genome is not yet complete, preliminary data were successfully used to identify and characterize a new type IV prepilin peptidase of V. cholerae, PilD. This prepilin peptidase is distinctly different from a previously described peptidase, TcpJ, showing only 25% identity at the amino acid level. This difference reflects the specificity for protein substrates. TcpJ appears to be responsible solely for processing of the type IV-B pilin protein TcpA (28), while PilD has a multitude of type IV-A substrates, including Eps proteins, essential for CT and HAP secretion, Msh proteins, essential for hemagglutination, and possibly TcpB, a protein essential for TCP production. In this study, we demonstrated that the loss of pilD disrupts each of these processes and that these defects are due solely to the loss of pilD, since the defects could be complemented in trans.
Recently, Marsh and Taylor (32) directly demonstrated that V. cholerae pilD (vcpD) encodes a type IV prepilin peptidase. They showed that EpsI and MshA produced in E. coli are N-terminally processed only when coexpressed with PilD. This observation confirms our prediction that secretion and MSHA defects are due to the lack of processing of type IV secretion signals by PilD.
Like us, Marsh and Taylor (32) showed that pilD (vcpD) mutants are defective for toxin secretion and MSHA, as well as for infant mouse colonization. However, they were unable to distinguish the phenotypes observed from the growth defects exhibited by the pilD (vcpD) mutants (32). In this work, our isolation and characterization of mutants with enhanced growth rates enabled us to characterize the role of pilD with less consideration for growth defects. These mutants were compared to more slowly growing deletion mutants, with similar results, and we further demonstrated that the defects were complemented by the introduction of pilD on a plasmid. Thus, we can firmly conclude that pilD is essential for secretion, MSHA, and TCP production.
In addition to the characterization of pilD, this work sheds light on continuing questions regarding the mechanism of bacterial adherence. Since type IV pili are essential for adherence in P. aeruginosa and N. gonorrhoeae (7, 16, 27, 43), it seems plausible that PilA is assembled into a new pilus essential for adherence and colonization. Surprisingly, pilA mutations resulted in no defects in these processes either alone or in combination with a mutation in mshA. Further, pilA mutants are not required for adherence to solid substrates, disputing a role for adherence in the environment (58). At present there is no information about the role of the putative pilus. However, the location of its gene within an operon with pilD indicates that it is expressed both in vivo and ex vivo. pilD is required for CT secretion and TCP production and thus must be expressed in vivo, and it is essential for MSHA, a phenotype expressed by bacteria grown in cultures. Indeed, preliminary analysis of lacZ fusions to the pil operon showed that the expression of this operon is initiated in the mid-log phase, just as pilD mutants begin to show severe growth defects (Fig. 3 and data not shown). Thus, it is unlikely that pilA, pilB, and pilC are silent genes coincidentally present in an operon with pilD. The 100% conservation of the pilA sequence between the classical and El Tor biotypes also indicates that pilA is likely to be important for some aspect of V. cholerae biology.
What, then, is the nature of the V. cholerae adherence
factors mediating adherence to HEp-2 cells? One possible hint comes from the analysis of the classical mutant KFV5R. This mutant is a
spontaneously arising second-site suppressor of the slow-growth defect
in pilD kan insertion mutant KFV5. It has a defect in HEp-2 cell adherence that cannot be complemented in trans by
the wild-type pilD gene (Fig. 6B). Thus, an adhesion factor
must have been disrupted during the reversion process, allowing faster
growth. This lost protein may be a type IV protein. It is clear that
the loss of pilin subunits can lead to enhanced growth of
pilD mutants of N. gonorrhoeae (10),
and our ability to produce a pilD mutation only in the
pilA background of N16961Sm suggests that a similar mechanism may allow enhanced growth of pilD mutants of
V. cholerae. Analysis of more recent genomic data
obtained from The Institute for Genomic Research shows that at least
five additional type IV cleavable proteins are encoded by the
V. cholerae genome (56a). Loss of any of
these five proteins may have enhanced the growth of the pilD
mutant KFV5 while decreasing HEp-2 cell adherence. Systematic deletion
of each of the five corresponding genes will determine if any of these
proteins are essential for HEp-2 cell adherence.
The adherence factor lost may also be an outer membrane protein. Secretion mutants of V. cholerae, including pilD mutants, lose outer membrane proteins, particularly the putative adhesin OmpU (32, 44). However, the loss of OmpU probably does not cause the HEp-2 cell adherence defect in KFV5R, since the reversion process and complementation restored OmpU expression to KFV5R. Thus, another outer membrane protein may be essential for HEp-2 cell adherence. Sengupta et al. (45) showed that rabbit antisera raised against major outer membrane proteins are partially protective against V. cholerae challenge in infant mice. This observation argues that outer membrane proteins may play a role in intestinal colonization and adherence. Attempts to isolate outer membrane protein mutants by signature-tagged mutagenesis and in vivo colonization repeatedly identified genes required for TCP production (8). Thus, the nature of outer membrane proteins that may be essential for adherence could probably be identified only by screening of transposon mutants for defects in adherence in vitro. Such an approach has identified a 40-kDa outer membrane protein from V. cholerae O139 that shows decreased adherence and infant mouse colonization, although the disrupted gene has not yet been identified (5).
This work has demonstrated that genomic data coupled with experimentation can rapidly expand the understanding of bacterial pathogenesis. However, the successful identification of a second prepilin peptidase is juxtaposed to the inaccurate supposition that pilA encodes a major adherence factor. These observations highlight the importance of genetic experimentation for complementing genomic data to fully enrich the fields of prokaryotic biology and eukaryotic biology.
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ACKNOWLEDGMENTS |
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We thank Ronald Taylor for gifts of plasmids and strains. We thank Michael Starnbach and his research group for gracious sharing of tissue culture facilities, supplies, and knowledge. The members of the Mekalanos laboratory are thanked for their ideas and suggestions; in particular, we thank Barry Wanner for helpful hints on constructing the mutants for this paper. We thank the Microbiology Sequencing Core Facility for providing additional sequence data for the pil gene cluster.
This research was supported by grant AI-18045 from the National Institutes of Health, and K.J.F. was supported by National Research Service Award training grant AI-07410.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology and Molecular Genetics, Harvard Medical School, Building D1-427, 200 Longwood Ave., Boston, MA 02115. Phone: 617-432-1935. Fax: 617-738-7664. E-mail: jmekalanos{at}hms.harvard.edu.
Editor: D. L. Burns
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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