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Journal of Bacteriology, July 1999, p. 4154-4160, Vol. 181, No. 14
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Division of Molecular Biology and
Biochemistry, School of Biological Sciences, University of
Missouri
Kansas City, Kansas City, Missouri 64110
Received 3 February 1999/Accepted 4 May 1999
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ABSTRACT |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The human pathogen Eikenella corrodens synthesizes type IV pili and exhibits a phase variation involving the irreversible transition from piliated to nonpiliated variants. On solid medium, piliated variants form small (S-phase), corroding colonies whereas nonpiliated variants form large (L-phase), noncorroding colonies. We are studying the molecular basis of this phase variation in the clinical isolate E. corrodens VA1. A genomic fragment encoding the major type IV pilin was cloned from the S-phase variant of strain VA1. Sequence analysis of the fragment revealed four tandemly arranged potential open reading frames (ORFs), designated pilA1, pilA2, pilB, and hagA. Both pilA1 and pilA2 predict a type IV pilin. The protein predicted by pilB shares sequence identity with the Dichelobacter nodosus FimB fimbrial assembly protein. The protein predicted by hagA resembles a hemagglutinin. The region containing these four ORFs was designated the pilA locus. DNA hybridization and sequence analysis showed that the pilA locus of an L-phase variant of strain VA1 was identical to that of the S-phase variant. An abundant pilA1 transcript initiating upstream of pilA1 and terminating at a predicted hairpin structure between pilA1 and pilA2 was detected by several assays, as was a less abundant read-through transcript encompassing pilA1, pilA2, and pilB. Transcription from the pilA locus was nearly indistinguishable between S- and L-phase variants. Electron microscopy and immunochemical analysis showed that S-phase variants synthesize, export, and assemble pilin into pili. In contrast, L-phase variants synthesize pilin but do not export and assemble it into pili. These data suggest that a posttranslational event, possibly involving an alteration in pilin export and assembly, is responsible for phase variation in E. corrodens.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Eikenella corrodens is a gram-negative human pathogen (10) that can cause endocarditis (6, 16), a variety of soft tissue and wound infections (10, 15, 20, 30), and other opportunistic infections. This bacterium has also been associated with periodontal diseases (4, 33, 37), although a causal role has not been clearly established. Despite increasing recognition of its role in disease, as reflected in growing numbers of case studies and clinical reports, little is known about the molecular factors that contribute to E. corrodens pathogenicity and virulence.
Most strains of E. corrodens exhibit an irreversible phase variation that is reflected in colony morphology changes. On solid medium, small (S-phase), so-called corroding, and large (L-phase), so-called noncorroding colonies are observed (11, 23, 28, 46). The L-phase variants arise from S-phase variants at a frequency much greater than mutation rates (24). Colony morphology and phase variation correlates with the presence of pili on S-phase variants and the absence of pili on L-phase variants (22, 23). In terms of piliation, phase variation in E. corrodens resembles the phase variation exhibited by pathogens such as Neisseria gonorrhoeae (7, 36, 50, 51) and Moraxella bovis (18, 34). In the latter species, the phase variation typically involves genomic recombination or mutagenic events that directly affect pilin synthesis or pilus assembly. Given that pili can be determinants of pathogenesis (1, 8, 31, 47), and that modulation of piliation may represent a mechanism to evade host immune response (9, 45, 49), the molecular basis of phase/antigenic variation is of considerable interest.
The pathogens mentioned above, as well as other gram-negative bacterial species, synthesize type IV pili (1, 14, 47). These pili are composed primarily of type IV pilin, a protein which ranges from 150 to 165 amino acids in length. Type IV pilin is synthesized as a precursor form (prepilin) that contains a basic leader sequence of variable length (4 to 25 residues). Following translation, the prepilin is cleaved at an atypical site by a cognate peptidase that simultaneously methylates the resultant amino-terminal amino acid, which is typically a phenylalanine residue. Following processing, the mature pilin is exported to the cell surface by a specific transport mechanism and assembled into pili. Class A type IV pilins from different species share a highly conserved, 30- to 32-residue hydrophobic amino-terminal domain that functions in protein-protein interactions during pilus assembly (47). The remainder of the mature pilin protein is less conserved and contains the major antigenic determinants.
We are examining the molecular basis of the pilus-associated phase variation exhibited by E. corrodens. Recently, we characterized the major pilus protein of clinical isolate strain VA1 and confirmed that the observed pili were type IV (27). Although genes encoding type IV pilin have also been cloned from two other E. corrodens strains (39, 53), their expression and potential role in phase variation have not been defined. In this report, we document the structure and expression of the major type IV pilin gene in S- and L-phase variants of strain VA1. Analyses of pilin gene expression and pilin processing suggest that a posttranslational event, possibly involving an alteration in pilin export and/or assembly, is responsible for phase variation in E. corrodens.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Bacterial strains and culture conditions.
The strains and
plasmids used in this study are listed in Table
1. E. corrodens VA1 is a
clinical isolate obtained from the Veterans Administration Medical
Center, Kansas City, Mo. (12). Strain VA1 forms both S- and
L-phase colonies on solid medium. Strains VA1-S1, VA1-S2, and VA1-S3
are independent S-phase isolates of strain VA1 that form S-phase
colonies and exhibit typical frequencies of phase variation to L-phase
colonies. Strain VA1-L2 is an L-phase isolate of VA1 that forms only
large colonies. E. corrodens was cultured aerobically at
35°C on chocolate agar plates purchased from Remel (Lenexa, Kans.).
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was used as the host for general
cloning vectors. E. coli BL21(D3) was used as the host for
pET-22b-based protein expression vectors. Both strains were propagated
in liquid or in solid Luria-Bertani medium with antibiotics at standard concentrations (5).
DNA methods.
Restriction endonucleases and modifying enzymes
were purchased from Promega (Madison, Wis.).
[-32P]dCTP was purchased from ICN (Costa Mesa,
Calif.). [
-32P]ATP and [35S]dATPS
were purchased from Amersham (Arlington Heights, Ill.). DNA
manipulations, including restriction digests, agarose gel electrophoresis, ligations, PCR amplifications, transformation of
E. coli, and plasmid minipreparations, were performed by
established protocols (5, 43). E. corrodens
genomic DNA was prepared by the procedure described for E. coli in reference 43 or with a kit from Qiagen
(Chatsworth, Calif.). For DNA hybridization analysis, digested DNA was
transferred to a charged nylon membrane (Hybond-N+;
Amersham) by the method of Reed and Mann (41). A DNA probe encompassing the pilA locus of strain VA1 (3.9-kbp
EcoRI fragment from plasmid pEC114) was generated from the
gel-purified fragment by random-primer labeling with a kit from
Promega. DNA hybridizations were performed at 58°C as described by
Sambrook et al. (43).
Cloning and sequencing of the pilA locus.
Total
DNA from strain VA1-S1 was partially digested with Sau3A,
and the digestion products were size fractionated by NaCl gradient
centrifugation and purified. To generate a subgenomic library, DNA
fragments in the range of 15 to 20 kbp were ligated into the
BamHI site of phage 
GEM11. The phage library was screened by hybridization to a probe for the pilE1 gene (1.4-kbp
SmaI fragment from plasmid pVD203) from N. gonorrhoeae MS11 (7), which was kindly provided by M. Koomey. One strongly hybridizing clone was identified, isolated, and
designated EP101. Mapping and DNA sequence analyses showed that a
terminal 0.6-kbp EcoRI-XhoI fragment from the
EP101 genomic insert contained sequences predicting a type IV
pilin-like gene. In a genomic DNA hybridization analysis, the 0.6-kbp
fragment identified a single 3.9-kbp EcoRI fragment of strain VA1-S1 total DNA. To clone the latter fragment, genomic DNA from
strain VA1-S1 was digested with EcoRI and size fractionated on an agarose gel. Fragments in the range of 3.9 kbp were eluted from
the gel and ligated into the EcoRI site of vector
pGEM-3Zf(
) (Promega), and the ligation products were used to
transform E. coli DH5. The transformants were screened
for plasmids containing pilin-like sequences by hybridization against
the 0.6-kbp EcoRI-XhoI fragment from EP101, using
a colony screening method (5). Plasmid pEC114, which
hybridized to the 0.6-kbp probe and contained the predicted 3.9-kbp
insert, was chosen for further analysis.
DNA sequence analysis. Double-stranded DNA sequencing templates were isolated and purified with a kit from Promega. Double-stranded sequencing of the 3.9-kbp EcoRI fragment of pEC114 was performed by the dideoxynucleotide chain termination method (44), using both manual and automated procedures. Manual sequencing was performed with Sequenase version 2.0 modified T7 DNA polymerase purchased from United States Biochemical (Cleveland, Ohio). Automated sequencing was performed on an Applied Biosystems (Foster City, Calif.) model 377 sequencer with AmpliTaq DNA polymerase. Sequencing reactions were primed with M13 universal primers or oligonucleotides synthesized on an Applied Biosystems model 381A oligonucleotide synthesizer. A portion of the pilA locus of strain VA1-L2 was sequenced from a PCR amplification product obtained by using primers 105-R3 (5'-GCCAGCTATTGCAGAATA-3') and 107-R7 (5'-TGCACCACTTCAAACCG-3'), corresponding to sequences determined from pEC114. DNA and protein sequences were analyzed and compared with sequences in the GenBank database by using MacVector (Oxford Molecular Group, Campbell, Calif.) and BLAST (2) sequence analysis programs.
RNA methods. Total RNA was isolated from S- and L-phase variants by using an RNeasy kit (Qiagen). Contaminating DNA was digested with RNase-free DNase, and the RNA was further purified by passage through an RNeasy column. For hybridization analysis, RNA samples were denatured, separated by electrophoresis on 1.2% agarose gels (43), and transferred to Hybond-N+ according to the manufacturer's instructions. The blots were hybridized with radioactive sense or antisense transcripts specific for pilA1 (generated from pEC203) or pilA2 (generated from pEC205), using the Riboprobe system (Promega). RNA hybridizations were performed at 42°C as described by Ausubel et al. (5).
Reverse transcriptase PCR. Single-stranded cDNA was synthesized from total RNA with an avian myeloblastosis virus reverse transcriptase system (Promega), using oligo(dT) or random primers. A negative control without reverse transcriptase was performed. An aliquot of the reaction volume was amplified by PCR using Taq polymerase (Promega) and the pilA locus-specific primers 105-R1 (5'-TGTTATCGCCATTATCGG-3'), 107-R3B (5'-AAATCCCTCAACGCTTGG-3'), 107-F3 (5'-AGAAGCAACTCGCTTTACCC-3'), RH-2 (5'-GGCAACTTGATGGCAAATATCCTAC-3'), 107-R6 (5'-TGTAAAGGGTTTGGGTGCC-3'), RH-3 (5'-GGCACCCAAACCCTTTACAAG-3'), and 107-R7 (5'-TGGACCACTTCAAACCG-3'). The PCR amplification products were transferred to Hybond-N+ membranes and hybridized to antisense RNA probes for pilA1 and pilA2 as described above.
Primer extension.
cDNA was synthesized with an avian
myeloblastosis virus reverse transcriptase primer extension system
(Promega) using primer 105-F1 (5'-CAAAATACCGATAATGG-3';
complementary to nucleotides 538 to 555 at the 5' end of
pilA1), which was end labeled with [-32P]ATP by using T4 polynucleotide kinase
(5). The primer extension products were analyzed against a
sequencing ladder on a denaturing polyacrylamide (8% acrylamide) gel.
Cell fractionation.
Cell fractionation was performed
essentially as described for E. coli by Studier et al.
(48). Cells from plates were suspended in 0.1 ml of buffer
(50 mM Tris [pH 8.0]), vigorously mixed in a vortex mixer for 30 s to shear pili, and then pelleted by centrifugation at
12,000 × g. The supernatant (surface fraction)
contained proteins, including pilin, that are bound and/or loosely
associated with the cell surface. To prepare the soluble and insoluble
fractions, the pelleted cells were resuspended in 0.1 ml of buffer,
brought to 2 mM EDTA, 0.1 mg of lysozyme per ml, and 0.1% Triton-X100, and incubated for 15 min at 30°C. The suspension was then sonicated (5-s pulse interval) for 1 min on ice and centrifuged at
12,000 × g. The resultant supernatant (soluble protein
fraction) and pellet (insoluble protein fraction) were isolated for
analysis. All protein fractions were mixed with sodium dodecyl
sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) sample buffer and
stored at 20°C.
Production of PilA1 antisera. The region of pilA1 encoding residues 26 to 146 of mature PilA1 was amplified from pEC114 by PCR using the following primers to produce flanking NcoI and XhoI sites: RH-4 (5'-GGCTTCCATGGACTACACTGCCCGTGCT-3') and RH-6 (5'-CTAACTCGAGTTGGCAGCTAGTTGGCAGACGG-3'). The PCR product was digested with NcoI and XhoI and ligated into expression vector pET-22b. The resulting plasmid, designated pEC206, provides for expression of a truncated PilA1 protein containing the added sequence LEH6, at the carboxyl terminus. Plasmid pEC206 was used to transform E. coli BL21(D3), and the His-tagged recombinant PilA1 protein was expressed, isolated, and purified by Ni-nitrilotriacetic acid (Qiagen) chromatography according to the manufacturer's instructions. A rabbit polyclonal antiserum was raised against the purified PilA1 protein by Atlantic Antibodies (Windham, Maine).
SDS-PAGE and immunoblot analysis. Protein samples were separated by SDS-PAGE on 20% polyacrylamide gels. Following electrophoresis, proteins were transferred to a nitrocellulose membrane (Nitrobind; Micron Separations Inc., Westborough, Mass.) as described by Ausubel et al. (5). The blots were blocked and incubated with the PilA1 antiserum (1:5,000). Bound antibodies were visualized following incubation of the blots with goat anti-rabbit immunoglobulin G (1:5,000) conjugated to alkaline phosphatase (KLC Laboratories, Gaithersburg, Md.) according to the manufacturer's instructions.
Electron microscopy. Negative staining and immunogold electron microscopic examination of whole cells were performed as described (27), using a polyclonal antiserum (1:1,000) prepared against pilin purified from strain VA1-S3.
Nucleotide sequence accession number. The complete DNA sequence of the pilA locus has been deposited in the GenBank database under accession no. AF079304.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Sequence analysis of the pilA locus. Plasmid pEC114 contains the 3.9-kbp EcoRI fragment of strain VA1-S1 genomic DNA that was identified by DNA hybridization against the pilE1 gene from N. gonorhoeae MS11. DNA sequence analysis revealed four potential open reading frames (ORFs) arranged in tandem on the pEC114 insert (Fig. 1). The first ORF (nucleotide positions 484 to 943) and second ORF (nucleotide positions 1013 to 1460) predict proteins of 153 and 149 residues, respectively. A BLAST search of the GenBank database showed that both ORFs predict obvious type IV pilins. On the basis of this identity, we designated the first ORF pilA1 and the second ORF pilA2. These and the subsequent gene designations are consistent with recommended bacterial gene nomenclature (17). The predicted PilA1 and PilA2 proteins respectively contain eight- and six-residue amino-terminal leader sequences upstream of the conserved phenylalanine that is presumed to represent the amino terminus of each mature protein. In comparison, the mature PilA1 and PilA2 proteins share 57% overall sequence identity and 87% sequence identity among their 32 amino-terminal residues. The predicted PilA1 amino-terminal sequence matched the amino-terminal sequence determined earlier for pilin of intact pili isolated from cells of strain VA1-S3 (27), demonstrating that PilA1 is the predominant pili component for this strain.
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pilA locus structure in phase variants. To examine a potential pilA-related genomic basis for their differential piliation, the structure of the pilA locus in E. corrodens S- and L-phase variants was examined by DNA hybridization analysis. Total DNA from strains VA1-S2 and VA1-L2 was digested with PvuII and BglII, PvuII, or PvuII and DraI and hybridized to the 3.9-kbp pEC114 insert (Fig. 2). For each digest, the hybridization profile obtained for strain VA1-S2 was indistinguishable from that obtained for VA1-L2 (Fig. 2; compare lanes 1 and 2). Identical results for S- and L-phase variants were obtained with other restriction enzymes. No hybridizing genomic fragments other than those originating from the pilA1 locus were observed. A similar analysis for other S- and L-phase variants yielded identical results (data not shown). In a related effort, the sequence of a 1.5-kbp region of strain VA1-L2 genomic DNA encompassing pilA and pilB was determined. When compared, the strain VA1-L2 sequence was found to be identical to that for strain VA1-S1 (data not shown).
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Pilin gene expression in phase variants. To characterize differential piliation between S- and L-phase variants at the level of pilin gene expression, transcripts from pilA1 and pilA2 in both variants were examined by RNA hybridization analysis. Total RNA isolated from cells of strains VA1-S1 and VA1-L2 was hybridized to RNA probes specific for pilA1 or pilA2 (includes pilB sequences). Similar hybridization profiles were obtained for both variants: the pilA1 probe detected an abundant 0.6-kb transcript and a less abundant 1.5-kb transcript (Fig. 3A), while the pilA2 probe detected a 1.5-kb transcript (Fig. 3B). Transcripts from pilA1 and pilA2 were also examined in two additional S-phase variants (strains VA1-S2 and VA1-S3) and two additional L-phase variants (strains VA1-L1 and VA1-L3), yielding identical results (data not shown). The 0.6-kb transcript is predicted to include pilA1 sequences, whereas the 1.5-kb transcript is predicted to include pilA1, pilA2, and pilB sequences. For both probes, the relative hybridization signal intensity was lower for strain VA1-L2 (Fig. 3; compare lanes 1 and 2). Replicate experiments showed that the pilA1 and pilA1A2B transcript levels in L-phase variants ranged from 43 to 80% of those in S-phase variants. Despite this difference, these results support transcription of the pilA locus in strain VA1-L2 and, coupled with pilin localization studies (see below), suggest a posttranscriptional basis for the lack of piliation in L-phase variants.
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70
consensus promoter sequences and a potential 54
consensus promoter sequence are located immediately upstream of the
identified guanine (Fig. 4). Located
further upstream is a 40-bp AT-rich region. A similar analysis of the
region between pilA1 and pilA2 did not reveal
potential promoter sequences; however, a 25-bp region (nucleotides 968 to 993) predicted to form a near-perfect hairpin was detected.
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Pilin localization in phase variants. The experiments described above indicated that both S- and L-phase variants express intact pilA1 transcripts. To define a cellular basis for the lack of piliation among L-phase variants, we examined the synthesis and localization of PilA1 in both S- and L-phase variants. Surface, soluble, and insoluble protein fractions were isolated from strains VA1-S1 and VA1-L2 and analyzed for PilA1 content by using a PilA1-specific antiserum. The strain VA1-S1 surface fraction, which should include pilin from pili and pilin loosely associated with the cell surface, contained a considerable amount of mature PilA1 (Fig. 5, lane 1). In contrast, no PilA1 was detected in the surface fraction of strain VA1-L2 (lane 2). Comparable amounts of mature PilA1 were detected in the soluble fraction of both strains (compare lanes 3 and 4). Similarly, the insoluble fraction of both strains contained comparable amounts of mature PilA1 (compare lanes 5 and 6). In addition to mature pilin, the insoluble fraction of both strains contained a unidentified 19-kDa immunoreactive protein (lanes 5 and 6). Control assays with different pilA1 and pilA2 mutants indicated that the 19-kDa immunoreactive species is ubiquitous to the insoluble fraction and is not a form of pilin. No PilA1 was detected in the periplasmic fraction of either strain VA1-S1 or strain VA1-L2 (data not shown). Collectively, these data suggest that the lack of piliation in L-phase variants is due to a posttranslational event, possibly involving PilA1 export and/or pilus assembly.
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Piliation of phase variants. Previous reports have described differential piliation among S- and L-phase variants of E. corrodens (22, 23). However, this phenomenon was not well documented, and subsequent studies have questioned the presence of pili on E. corrodens (32, 38). To document their differential piliation, cells of strains VA1-S3 and VA1-L2 were examined by immunogold electron microscopy using a polyclonal antiserum raised against pilin purified from strain VA1-S1 (27). In an analysis of over 200 strain VA1 cells, we detected one or more immunoreactive pili on 47% of the strain VA1-S3 cells but on none of the strain VA1-L2 cells. Furthermore, no immunoreactive material was observed on the cell surface of either strain. A representative electron micrograph for strains VA1-S3 and VA1-S2 is presented in Fig. 6. In a similar analysis of over 200 E. corrodens ATCC 23834 cells, immunoreactive pili were detected on all of the S-phase cells and none of the L-phase cells.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The gram-negative pathogen E. corrodens elaborates type IV pili and exhibits a phase variation involving an irreversible transition from piliated to nonpiliated cells. To initiate an investigation into the molecular basis of this transition event, we have cloned and characterized the pilA locus from E. corrodens VA1. The pilA locus includes four putative genes arranged in tandem. The first two genes, designated pilA1 and pilA2, each encode a type IV pilin. The third gene, designated pilB, encodes a potential pilus assembly protein, whereas the fourth gene, designated hagA, encodes a putative hemagglutinin. In terms of the pilin and hemagglutinin genes, the strain VA1 pilA locus structurally resembles the similar locus described for E. corrodens ATCC 23834 (39) (see below). However, the strain VA1 pilA locus differs from the strain ATCC 23834 locus by the presence of pilB. Given that DNA hybridization analyses of genomic DNA using heterologous and homologous probes failed to detect additional hybridizing fragments, pilA1 and pilA2 most likely represent the only type IV pilin genes present in strain VA1.
This study showed that S- and L-phase variants of E. corrodens are identical with respect to pilA1 and pilA2 structure and sequence. This differs from what is most commonly observed for the best-characterized bacterial pathogens exhibiting a similar phase and/or antigenic variation that involves expression of type IV pilin. Among these are N. gonorrhoeae and N. meningitidis, which possess one or two pilin (pilE) genes and a variable number of silent partial pilin (pilS) genes. For these strains, phase variation can be achieved by spontaneous mutations in pilE, which results in nonpiliated cells (7, 50, 51). In addition, irreversible intragenic recombination events involving the pilE and pilS genes result in the synthesis of structurally altered pilins, giving rise to antigenic variation (19, 36, 45, 52). Another example is M. bovis, in which two different pilin genes (fimL and fimQ) are alternatively expressed by means of a DNA inversion that links one or the other gene to a single common promoter (18, 34). Thus, the most common phase and/or antigenic variation exhibited by N. gonorrhoeae, N. meningitidis, and M. bovis results from a genomic mutation or recombination events directly involving type IV pilin genes. In comparison, the phase variation exhibited by E. corrodens is unique in that it does not involve a pilin gene-associated mutation or genomic recombination event.
The RNA hybridization analysis indicated that transcripts from
pilA1, but not pilA2, were abundant in both S-
and L-phase variants of strain VA1, consistent with previous work
showing that PilA1 was the major pilus protein for this strain
(27). The 5'-end mapping and sequence analyses suggest that
the abundant pilA1 transcript originates from a
70-type promoter located 200 bp upstream of the putative
PilA1 translation initiation codon. If correct, the 0.6-kb
pilA1 transcript terminates at the pilA1-pilA2
intergenic region, the sequence of which predicts a potential hairpin
structure. A low-abundance 1.5-kbp transcript that hybridized to probes
for both pilA1 and pilA2 was also detected in the
S- and L-phase variants. This larger transcript is most likely the
product of transcription from the pilA1 promoter through the
pilA1-pilA2 intergenic region, giving rise to a
pilA1A2B polycistronic message. Presumably, the predicted
hairpin structure between pilA1 and pilA2
represents the terminator component of a transcription attenuation
mechanism. Such an attenuation mechanism would provide for controlled
expression of pilA1, pilA2, and pilB
as required for pilus formation and resembles a similar mechanism that
has been proposed for D. nodosus (25).
The detection of transcripts from pilA1 and pilA2 in the L-phase variant of strain VA1 was somewhat unexpected. In the absence of a detectable pilin gene-associated recombination or mutagenesis event, it was hypothesized that the phase variation exhibited by strain VA1 might be achieved through differential expression of pilA1 or pilA2. The abundance of both the 0.6-kb pilA1 transcript and 1.5-kb pilA1A2B transcript was consistently lower in L-phase variants; however, this difference was deemed insufficient to account for their lack of piliation. We suspect that the decreased level of the pilA1 and pilA1A2B transcripts is related to factors associated with extraction of RNA from the morphologically distinct L-phase variants, as opposed to factors associated with transcription. Collectively, the pilA1 and pilA2 structure and transcription data support a posttranscriptional basis for the nonpiliated phenotype of the L-phase variants.
The pilin localization studies revealed that L-phase variants are not compromised in pilin biosynthesis but that they differ from S-phase variants with respect to the fate of synthesized pilin. For both S- and L-phase variants, similar levels of mature PilA1 were detected in the insoluble protein fraction. Because this fraction includes the cytoplasmic membrane and associated components, the presence of mature PilA1 is consistent with studies of Pseudomonas aeruginosa and other species showing that initial processing of type IV pilins (leader sequence cleavage and amino-terminal methylation) is accomplished on the cytoplasmic surface of the cytoplasmic membrane by membrane-associated cognate prepilin peptidases (47). Moreover, the similarity in pilin composition of the insoluble protein fractions suggests that initial processing of PilA1 is not significantly altered in the L-phase variants. The S- and L-phase variants were also indistinguishable in the PilA1 composition of their soluble protein fractions, as similar levels of mature PilA1 were detected for both. In contrast to these results is the PilA1 composition of the surface protein fraction: whereas mature PilA1 was readily detected in the S-phase variant surface protein fraction, none was detected in the corresponding fraction from the L-phase variant. This lack of pilin in the L-phase variant surface fraction is consistent with the immunogold electron microscopic analysis showing that only S-phase variants possessed intact pili. On the basis of these data, we conclude that an altered pilin posttranslational event, possibly involving one or more steps in pilin export and/or assembly, is responsible for the lack of piliation associated with the L-phase variants of E. corrodens VA1.
The specific stage or event in export or assembly of pili that might be affected in the L-phase variants is not known. In general, the pathway for processing, export, and assembly of type IV pilins is not well defined. Perhaps the best-characterized type IV pilus biosynthetic pathway is that of P. aeruginosa, for which more than 22 genes involved in pilin expression and/or pilus assembly and function have been identified by transposon tagging (35). More than half of these genes appear to be directly involved in pilus assembly and function and are thought to represent a subset of a general system for the formation of surface-associated protein complexes (26). Of particular interest is the observation that mutations in the individual genes in this subset result in the lack of piliation. Homologs to many of the putative pilus assembly genes have been identified in other type IV piliated bacteria, supporting a common mechanism for processing, export, and assembly of type IV pili. Presumably, E. corrodens shares this mechanism; if this is so, events that affect one or more of the corresponding genes might be involved in the transition from S- to L-phase variants. Experiments to examine this possibility are in progress.
A precedence for phase variation mediated by a type IV pilin-associated posttranslational event has been established for N. gonorrhoeae MS11. This strain, like most examined N. gonorrhoeae strains, contains two unlinked copies of the pilC gene (not a P. aeruginosa pilC homolog), designated pilC1 and pilC2, which encode a protein involved in pilus assembly (29). Only pilC2 is expressed in piliated MS11 cells due to a translational frameshift in pilC1. Spontaneous phase variation of MS11 cells is achieved by frameshift mutations in a run of G residues within the region of pilC2 encoding the signal peptide of PilC, abolishing translation of the protein. Pilin synthesis is maintained in the absence of PilC, but no pili are assembled. In this regard, the strain MS11 pilC2 mutants and the L-phase variants of E. corrodens VA1 are phenotypically indistinguishable. Whether E. corrodens VA1 possesses a homolog to pilC from N. gonorrhoeae remains to be examined; however, we note that thus far, PilC appears to be unique to N. gonorrhoeae (47). A significant difference between the pilC2-based phase variation in N. gonorrhoeae MS11 and the phase variation in E. corrodens VA1 is that the former is reversible. Piliated revertants to strain MS11 pilC2 mutants are readily obtainable; the reversion involves mutations in pilC1 or pilC2 that result in translation of PilC. In contrast, no L- to S-phase revertants of E. corrodens VA1 have been observed. Given these data, we predict that the putative posttranslational basis of phase variation in E. corrodens VA1 differs mechanistically from pilC2-based phase variation in N. gonorrhoeae.
Genes encoding type IV pilins have been cloned from two other E. corrodens strains, ATCC 23834 (39) and ATCC 31745 (53). A feature common to these two strains and strain VA1 is the presence of two tandemly arranged type IV pilin genes separated by 70 to 80 bp. The strain ATCC 23834 pilin genes are designated ecpA and ecpB (39), whereas the strain 31745 pilin genes are designated ecpC and ecpD (53). For the strain VA1 pilin genes pilA1 and pilA2, we adopted the designations of the P. aeruginosa pilin gene system (1), which is consistent with recommendations for bacterial gene nomenclature (17). The six predicted pilins share 80 to 97% sequence identity at their amino termini (first 32 residues of the mature protein), which is typical for all examined type IV pilins (47). Overall, the six predicted pilins share 35 to 43% sequence identity, which is consistent with the reported decreased sequence conservation within the carboxyl regions of type IV pilins (47). In general, the two pilins from a given strain share greater overall sequence identity with each other than with pilins from another strain, suggesting that for each strain, the pilin gene pairs arose by a duplication event. The G+C contents of pilA1 and pilA2 (47.9 and 40.1%, respectively) significantly differ from the genomic G+C contents (53 to 58%) reported for several different E. corrodens strains (13, 28, 42), suggesting that the pilin gene(s) may have been acquired by horizontal transfer. Since these are characteristics of a variety of virulence genes acquired by intra- and interspecies gene transfer in bacterial pathogens (21, 54), the pilA locus may represent an acquired region encoding pathogenicity-associated proteins.
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ACKNOWLEDGMENTS |
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We thank D. Mason for help in the initial cloning of the E. corrodens pilA locus, D. Law and staff for assistance with electron microscopy, and W. Thomas and staff for assistance with DNA sequencing.
This research was partially supported by Public Health Service grant DE10439 (R.L.H.) from the National Institutes of Health.
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FOOTNOTES |
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*
Corresponding author. Mailing address: University of
MissouriKansas City, School of Biological Sciences, 5100 Rockhill
Road, Kansas City, MO 64110. Phone: (816) 235-2573. Fax: (816)
235-5595. E-mail: schaeferm{at}umkc.edu.
Present address: Center for Scientific Review, National Institutes
of Health, Bethesda, MD 20892.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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