Insertional Inactivation of Treponema denticola tap1 Results in a Nonmotile Mutant with Elongated Flagellar Hooks

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Limberger, R. J.
	Articles by Samsonoff, W. A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Limberger, R. J.
	Articles by Samsonoff, W. A.

Previous Article | Next Article

Journal of Bacteriology, June 1999, p. 3743-3750, Vol. 181, No. 12
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Insertional Inactivation of Treponema denticola tap1 Results in a Nonmotile Mutant with Elongated Flagellar Hooks

Ronald J. Limberger,^* Linda L. Slivienski, Jacques Izard, and William A. Samsonoff

David Axelrod Institute for Public Health, Wadsworth Center, New York State Department of Health, Albany, New York 12201-2002

Received 28 December 1998/Accepted 20 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The treponemal fla operon is comprised of numerous motility-related genes; however, the initial gene of this operon, tap1,has no known function. A recently developed system to generatespecific mutants in Treponema denticola was utilized to determineif Tap1 was essential for motility. T. denticola tap1 and flankingDNA were identified, cloned, and sequenced, and a suicide plasmidthat contained tap1 interrupted with an erythromycin resistancecassette (ermF and ermAM) was constructed. Because of potentialpolar effects from this cassette, a second plasmid that containedtap1 interrupted with a modified erythromycin resistance cassettethat lacked the putative ermF transcription terminator was constructed.Electroporation-mediated allelic exchange incorporated the interruptedtap1 genes into the T. denticola chromosome, creating Tap1-deficientmutants. Reverse transcriptase PCR revealed that the erythromycinresistance cassette within tap1 did not terminate fla operon transcriptionin either mutant. Moreover, the phenotypes of the two mutantswere indistinguishable. These mutants lacked motion in liquidculture, were unable to spread on agar plates, and lacked flagellarfilaments as determined by electron microscopy. Immunoblots revealeda marked reduction in detectable FlaB flagellar filament proteincompared to that of wild type; however, flaB RNA was easily detectable,and transcription levels did not appear to be altered. The basisfor the lack of filament protein expression is unknown. Immunoblottingalso showed that the flagellar hook protein (FlgE) was synthesizedin the Tap1-deficient mutant; however, electron microscopy revealedthat the mutant possessed unusual elongated hooks of variablelengths. We propose that treponemal Tap1 is analogous to FliK,which is involved in monitoring the flagellar hook length of Salmonellatyphimurium.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Treponema denticola is an anaerobic spirochete that is associated with periodontal disease (32, 33). As with all spirochetes,the structure and motility of T. denticola are unusual and enablemovement in highly viscous environments (17, 18). A uniquefeature of T. denticola (and all spirochetes) is the locationof the flagellar filaments within the periplasmic space, althoughunder certain conditions they may protrude from the cell (3,15). The T. denticola flagellar filaments are complex, consistingof three core proteins (FlaB1, FlaB2, and FlaB3) and a major sheathprotein, FlaA (29). However, the general structure of the flagellumappears similar to that of other bacteria, since it consists ofa basal body, rod, flagellar hook, and filament (25, 29).In contrast to the structural similarities, DNA sequencing andtranscription studies have clearly shown that the organizationand expression of motility genes are unique in the spirochetes(7-10, 12, 13, 22).

Motility of spirochetes is complex and likely requires approximately 50 genes, many of which are organized into several largeoperons (7-10, 12, 13, 22). The extensive treponemal flaoperon in Treponema phagedenis and Treponema pallidum comprisesgenes directly associated with motility, including the flagellarhook gene (flgE) and flagellar motor genes (motA and motB), inaddition to genes of unknown function (tap1) (12, 22). Previousstudies have shown that T. phagedenis Tap1 is a soluble proteinthat partitions in the aqueous phase during Triton X-114 extractionand is associated with motility, because tap1 is the first geneof the fla motility operon (22). However, there has been nodirect evidence for a role of tap1 in the motility oftreponemes.

Genetic analysis of T. denticola, like that of other spirochetes, has been hampered by a paucity of genetic tools for analysis.Recently, Li et al. showed that a gene cassette that includesermF and ermAM in tandem (ermF-ermAM) conferred erythromycin resistancein T. denticola (ermF) and also in Escherichia coli (ermAM) (19).This cassette was inserted into flgE, and a specific mutant wascreated by electroporation-mediated allelic exchange of the insertionallyinactivated flgE. This nonmotile mutant lacked flagellar hooksand filaments, as determined by electron microscopy. Using immunoblotting,Ruby et al. revealed that this mutant was also deficient in flagellarfilament proteins (29). Specifically, FlaB polypeptides werenot detected and minimal amounts of FlaA were detected in theflgE-deficient mutant. These results demonstrated the utilityof the erythromycin resistance cassette in generating specificmutants foranalysis.

The ermF-ermAM cassette used by Li et al. was postulated by Fletcher et al. to have a potential transcription terminator locatedbetween ermF and ermAM (6). This terminator-like sequence wouldpotentially cause polar effects when inserted within an operon,but it is not known if the terminator is functional in T. denticola.For analysis of single genes of the fla operon, it is criticalto have a nonpolar cassette available for gene interruptions.Conceivably, removal of this putative terminator would permitthe erythromycin resistance cassette to be used to study singlegenes located within operons without affecting downstreamgenes.

Our goal was to identify the fla operon of T. denticola and interrupt the T. denticola tap1 gene with a nonpolar erythromycinresistance cassette to determine whether tap1 is involved in motility.We found that the organization of the T. denticola fla operonis similar to that for other treponemes, and interruption of T.denticola tap1 with a nonpolar cassette resulted in a nonmotilecell. The Tap1-deficient mutants possessed unusually long andvariable-length flagellar hooks, suggesting that Tap1 may be involvedin monitoring hook length, analogously to FliK of Salmonella typhimurium(14).

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Culture media and conditions, strains, and molecular methods. T. denticola (ATCC 33520) was grown in new oral spirochete medium (NOS) with 10% heat-inactivated rabbit serum and 10 µg ofcocarboxylase per ml at 36°C in an anaerobic chamber (Coy LaboratoryProducts, Inc., Grass Lake, Mich.) with an atmosphere of 85% nitrogen,5% carbon dioxide, and 10% hydrogen. For growth on semisolid media,0.5% agarose was included withNOS.

E. coli DH5 $alpha$ (Gibco BRL, Grand Island, N.Y.) was used for most transformations and was grown in Luria-Bertani (LB) broth at37°C with shaking. Nonmethylated plasmid DNA was prepared in E.coli SCS110 (Stratagene Corp., La Jolla, Calif.) for electroporationof T. denticola.

The PCR and reverse transcriptase PCR (RT-PCR) were performed with reagents and thermal cyclers available from Perkin-Elmer(Foster City, Calif.). Plasmid pCRII-TOPO was purchased from InvitrogenCorp. (Carlsbad, Calif.), and pUC19CAT, which contains a chloramphenicolresistance gene in pUC19, was a lab stock. Lambda ZAP Expresswas obtained from Stratagene. Ligations were performed eithervia rapid ligations (Boehringer Mannheim Corp., Indianapolis,Ind.) or traditional 16-h ligations with T4 DNA ligase (New EnglandBioLabs, Beverly, Mass.) or directly by the TOPO TA cloning system(Invitrogen). Total T. denticola RNA was isolated as previouslydescribed for T. phagedenis with materials available through Amresco(Solon, Ohio) (24). Plasmid minipreparation DNA was isolatedby standard techniques (26), and Qiagen Midi columns (QiagenCorp., Chatsworth, Calif.) were used for purification of largeramounts of DNA for transformation of T. denticola. Radioisotopeswere obtained from Amersham Life Sciences, Inc. (Arlington Heights,Ill.).

The ermF-ermAM cassette and a plasmid containing the T. denticola flgE gene interrupted with this cassette were kindly providedby Howard Kuramitsu (State University of New York,Buffalo).

Antiserum against T. pallidum recombinant FlgE was previously generated by mouse immunizations in our laboratory (20, 23).Rabbit antisera generated with T. phagedenis FlaB and FlaA polypeptideswere kindly provided by Nyles Charon (West Virginia University,Morgantown) (20).

Identification of the T. denticola fla operon. The 5' end of the T. denticola fla operon was identified by screening a Lambda ZAP Express library prepared by partial Sau3AIdigestion of T. denticola chromosomal DNA by previously describedmethods (24). The probe was a segment of flgE made by PCR ofT. denticola with a DNA sequence available from Li et al. (19)(GenBank accession no. L75953). DNA sequencing at the WadsworthCenter Molecular Genetics Core facility was done with the Perkin-ElmerABI Prism 377 and ABI 373A sequencers. In addition, approximately78 bp at the 3' end of flgE of T. denticola was previously determinedby amplification of this region by degenerate primer PCR and DNAsequencing (4, 5). Sequences were assembled and analyzedwith the Wisconsin package, version 9.1 (Genetics Computer Group,Madison, Wis.).

Primer extension. To identify the start site of transcription of the T. denticola fla operon, primer extension was performed. TDW13 (5'-CAGAGTCTTCTCTTTCCG-3')was labeled with ³²P by T4 polynucleotide kinase, and the primer extension reactionwas performed with the Primer Extension System (Promega Corp.,Madison, Wis.). In the extension reaction, 1 pmol of labeled TDW13was used. For determining the length of the primer extension products,a ³⁵S-labeled DNA ladder was generated by PCR with the control sequencefrom the AmpliCycle sequence kit (Perkin-Elmer) and the forwardM13 primer. The Burst-Pak sequencing gels were used (Owl Scientific,Inc., Woburn, Mass.) to prepare 6% polyacrylamide gels for electrophoresis.Autoradiography was performed with XAR-2 film (Eastman Kodak,New Haven, Conn.) at $-$ 70°C with an intensifyingscreen.

Construction of two plasmids containing T. denticola tap1 interrupted with modified erythromycin resistance cassettes. A DNA fragment containing T. denticola tap1 was prepared by PCR of T. denticola chromosomal DNA with primers TDW8 (5'-CTGATGAAGCCCGATTTG-3')and TDW5 (5'-GTTTACCTGCATAAACTACCTC-3') and ligated to pCRII-TOPO.A clone harboring the 1,230-bp insert was selected, the plasmidDNA was digested with EcoRI, and the insert DNA was ligated topUC19CAT. A clone containing the 1,230-bp insert of tap1 DNA wasdigested with BglII, which cut at a site 706 bp downstream fromthe start of the tap1 gene (see Fig. 1). Tap1 was then inactivatedby cloning the two erythromycin resistance cassettes into theBglII site as indicatedbelow.

Two different erythromycin resistance cassettes were constructed and used for insertional inactivation of T. denticola tap1.The first utilized the ermF-ermAM cassette described by Li etal. (19). To facilitate genetic manipulations, this cassettewas amplified from pHfLE (19) with the primers ERMBGLF (5'-TATAAGATCTCCGATAGCTTCCGCTATTGC-3')and ERMBGLR (5'-TATAAGATCTGAAGCTGTCAGTAGTATACC-3'), which bothcontain synthetic BglII sites, and then cloned into pCRII-TOPO.This plasmid was digested with BglII, and the 2.1-kb DNA product(ermF-ermAM cassette) was gel purified, phenol extracted, andethanol precipitated. The ermF-ermAM cassette was then ligatedinto the BglII-digested pUC19CAT plasmid that contained T. denticolatap1, transformed into E. coli DH5 $alpha$ , and plated on LB plates containing300 µg of erythromycin per ml. Erythromycin-resistant E. colicolonies were picked and grown in LB broth, and plasmid DNA wasisolated. Orientation of the tap1 gene and ermF-ermAM cassettewas determined by PCR and DNA sequencing; only those clones containingthe ermF-ermAM cassette oriented in the same direction as tap1were chosen for the insertional inactivation in T. denticola.

The second strategy involved construction of an erythromycin resistance cassette that did not contain putative transcriptionterminator or ermF promoter sequences. The ermF gene possessessequences resembling a transcription terminator following theend of the coding region (6). This terminator-like region,as well as DNA preceding the ermF region (including the ermF promoter),and some nonessential DNA flanking the ermAM gene were removedby the following procedure. An oligonucleotide primer that annealedjust upstream of the ribosome binding site of ermF and containeda synthetic BglII site was synthesized (ERFNEWF, 5'-TATAAGATCTATTATCCGCACCCAAAAAG-3')together with a second primer that anneals to the complementarystrand at the stop codon of ermF (ERFNEWR, 5'-TATACCCGGGCAACCACCCGACTTTGAACTA-3').A synthetic SmaI site was engineered into the second primer. Afteramplification from the pHfLE template DNA, this ermF gene wascloned into pCRII-TOPO and verified by DNA sequencing. This vectorcontaining ermF was digested with SmaI to open a blunt-end cloningsite just downstream of ermF. Next, ermAM was amplified with primersthat anneal just upstream of the regulatory region (ERAMNEWF,5'-GAAGCAAACTTAAGAGTGTG-3') and also near the stop codon of ermAM(ERAMNEWR, 5'-TATAAGATCTGAAGCTGTCAGTAGTATACC-3'). A syntheticBglII site was incorporated into ERAMNEWR. This fragment was bluntend ligated to the SmaI site of the pCRII-TOPO/ermF plasmid, transformedinto E. coli, and selected with 300 µg of erythromycin per ml.Proper orientation of the insert DNA was confirmed by PCR andDNA sequencing. The resulting clone had ermF and ermAM in tandemand no putative transcription terminator. This erythromycin resistancecassette was removed from the plasmid by digestion with BglIIand cloned into the BglII site of tap1 as indicated above forthe original ermF-ermAM cassette. This cassette that lacked theermF promoter and the putative transcription terminator was designatedermF-ermAMnp.

Insertional inactivation of T. denticola tap1 with the ermF-ermAM and ermF-ermAMnp cassettes. The protocol developed by Li et al. was used with some minor modifications for insertional inactivation of T. denticola (19).Briefly, 100 ml of T. denticola was grown to an optical densityof 0.3 at 600 nm. Cells were washed three times with cold 10%glycerol in water and resuspended in a final volume of 2 ml onice. Electroporation was done with 10 µg of linearized DNA witha Bio-Rad Gene Pulser at 1.8 kV, 200 $Omega$ , with 25 µF and a 0.1-cmcuvette. Time constants of 4.1 to 4.6 were considered optimal.After overnight incubation in 10 ml of NOS broth without erythromycin,plating was done on NOS containing 0.5% agarose and 20 µg of erythromycinper ml. Colonies usually were visible within 7 days. PCR and Southernblotting were used to determine that the wild-type tap1 gene wasreplaced with the insertionally inactivated tap1 gene by allelicexchange (21, 31).

Identification of T. denticola flaB. T. denticola contains three flaB genes (29). To obtain a partial sequence from one of these genes, primers from conservedregions of T. phagedenis flaB were used in a PCR amplificationof T. denticola (24). The primers FLAB2 (5'-GTGGTTCCATATCGGGGCC-3')and FLAB4 (5'-CCTGCAAAAAGTTTAGCGC-3') amplified a 620-bp fragmentof T. denticola DNA which was cloned into the pCRII-TOPO cloningvector and sequenced to confirm a flaBidentity.

Isolation of flagellar hooks and electron microscopy. Flagellar hooks were isolated by a modification of previously described methods (23). Approximately 10⁹ cells of T. denticola were washed twice with Tris-buffered saline,the outer sheath was removed with 2% Triton X-100, and the cellswere washed once with Tris-buffered saline. The final pellet wasresuspended in 10 mM sodium phosphate buffer and sonicated onice for 1 min at a 1-s cycle time and 50% duty cycle. DNase, RNase,and lysozyme (20 mg each) were added to the sonicate along withfinal concentrations of 0.05% Triton X-100, 0.02 mM EDTA, 2.5%glycerol, and 25 mM MgSO₄, and the mixture was incubated overnightat 4°C. Next, Triton X-100 was added to a final concentrationof 2% and the incubation was continued for 1 h at 20°C. The lysatewas centrifuged at 41,000 × g in an SW-28 rotor for 30 min througha gradient containing 100, 75, 50, and 25% glycerol. The viscousmaterial at the 75%-100% glycerol interface was collected anddialyzed overnight against water at 4°C. This fraction was enrichedfor flagellar hooks; some material was saved for electron microscopy,and the remainder was treated with pH 2.2 glycine buffer to removeany flagellar filaments as previously described (23).

For electron microscopic visualization of T. denticola cells, 1 ml of logarithmic-phase culture was centrifuged for 1 minat 10,000 × g. The pellet was resuspended in the same amount ofwater containing 1% Triton X-100 reduced, a chemically modifiedform of Triton X-100 (Aldrich Chemical Co., Milwaukee, Wis.),and incubated overnight at 4°C. The sample was centrifuged for1 min at 10,000 × g, and the pellet was resuspended in 100 µlofwater.

Negative staining was used to visualize cells or purified hooks. Drops (40 µl) of the sample were placed on dental wax. Formvar-coatedcopper grids were floated on the drops for 2 to 4 min; excessliquid was removed by wicking with filter paper, and the gridswere immediately washed by floating them on 2 drops of double-distilledwater. After the final wash, excess water was removed, the gridswere briefly floated on 2% sodium phosphotungstate (pH 7.0), liquidwas removed by wicking, and the samples were viewed in a Zeiss(LEO) 910 transmission electron microscope operating at 80keV.

Transcription analysis. RT-PCR was used to determine whether genes of the fla operon were transcribed (22). Northern blots are ineffective becausethe fla operon transcript is very large and the RNA transcriptis significantly degraded. For analysis of transcription by RT-PCR(see Fig. 1), primers for upstream of the ermF-ermAM cassetteinsertion within tap1 were TDW8 (5'-CTGATGAAGCCCGATTTG-3') andTDW9 (5'-TTTAGCAAATCCTTGGGC-3'), and primers for genes immediatelydownstream of the ermF-ermAM cassette were TDW12 (5'-CGGGAACAGTAACTGTTGCCTC-3')and TDW5 (5'-GTTTACCTGCATAAACTACCTC-3'). Primers located withinflgE were TDWFLGEF (5'-CGTTGCCAACGTAAATAC-3') and TDWFLGER (5'-AAATTCGGTAGACCAAGTAG-3').Oligonucleotide primers for detection of flaB RNA were TDWFLABF(5'-CTGCAAATAGGAGCATTGGAAC-3') and TDWFLABR (5'-GCTATTGTTATTAGCCTGAGCGAG-3').

Production of Tap1-MBP fusion protein, antiserum production, and immunoblotting. T. denticola tap1 was amplified with the primers TDWTAPF (5'-TATAGAATTCCAGGCTTTGCCGGTAAAAGAGC-3') and TDWTAPR (5'-TATACTGCAGGTTTACCTGCATAAACTACCTC-3'),which contains synthetic EcoRI and PstI sites, respectively. TDWTAPFanneals 21 nucleotides (nt) downstream of the ATG start codonof tap1, and TDWTAPR includes the native stop codon. After amplification,the 1,372-bp product was cloned into pCRII-TOPO. This plasmidwas then digested with EcoRI and PstI to liberate the fragmentcontaining tap1, which was ligated into pMAL-c2 (New England BioLabs).The ligation mixture was transformed into CaCl₂-competent E. coliDH5 $alpha$ , heat shocked, and plated on LB agar plates containing X-Gal(5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside) and IPTG (isopropyl- $beta$ -D-thiogalactopyranoside)as previously described (24). White colonies were picked, andclones with the proper insert were identified by restriction endonucleasedigestion followed by sequencing of the plasmid-insert junctions.Tap1-maltose-binding protein (MBP) fusion protein was inducedwith IPTG and purified over amylose resin by previously describedmethods (23). Immunization of rabbits with the Tap1-MBP fusionprotein and collection of antisera were done by Biodesign Inc.(Kennebunkport,Maine).

Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and immunoblotting were performed as previously described, and theblots were developed with alkaline phosphatase-labeled secondaryantibody (20). About 50 µg of each cell lysate was loaded perlane, and primary antisera were used at a 1:50 or 1:100dilution.

Nucleotide sequence accession number. The GenBank nucleotide sequence accession number for T. denticola tap1, flgD, and partial flgE is AF049342 and for partialflaB is AF072133.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Identification and molecular characterization of the T. denticola fla operon. After screening of the T. denticola Lambda ZAP Express library, one clone that possessed a 3,902-bp insert was obtained. Thiscloned DNA was sequenced in both directions with synthetic oligonucleotidesand revealed the 5' region of the T. denticola fla operon (Fig.1). As noted with other treponemal fla operons, T. denticola flabegins with tap1 (457 amino acids), followed by flgD, which isinvolved in flagellar hook assembly (169 amino acids) (28),and flgE, the flagellar hook protein (the first 237 amino acidswere deduced) (23). In addition, there is an open reading frameupstream of tap1 that is transcribed in the opposite directionfrom the fla operon; this is similar to the gene arrangement inT. phagedenis and T. pallidum (8, 22).

View larger version (12K):
[in this window]
[in a new window]

FIG. 1. Diagram of the fla operon organization of T. denticola and 5' upstream region. P_fla indicates the approximate location of the fla operon promoter. The ermF-ermAM cassette is indicated above the operon and is shown where it is inserted in the BglII site for creating Tap1-deficient mutants. The locations of primer pairs used for RT-PCR are indicated by arrows and are represented as follows: 1, TDW8; 2, TDW9; 3, TDW12; 4, TDW5; 5, TDWFLGEF; 6, TDWFLGER. Sequences of the primers are given in Materials and Methods.

Preceding tap1 is a sigma 28-like sequence (Fig. 2A) that is likely involved in transcription of the fla operon. Primer extensionanalysis revealed that the start site of transcription was located9 nt downstream of this promoter and 32 nt upstream from the ATGtranslational start site (Fig. 2B). The promoter sequence wasvery similar to the P_fla and sigma 28 sequences in othertreponemes (Fig. 3). RT-PCR also revealed that transcription proceededfrom P_fla through flgD and flgE, which confirmed theorganization of these genes into an operon (data not shown).

View larger version (53K):
[in this window]
[in a new window]

FIG. 2. Identification of the fla operon promoter. (A) DNA sequence including the proposed $-$ 10 and $-$ 35 regions of P_fla. The large arrow indicates the start site of transcription determined by primer extension. M indicates the first amino acid of the Tap1 polypeptide. (B) Primer extension assay to determine the start site of transcription of P_fla. A, C, G, and T indicate nucleotides used to generate a size ladder with unrelated DNA. Lanes 1 and 2 contain the primer extension reaction products of 2 and 5 µl, respectively.

View larger version (26K):
[in this window]
[in a new window]

FIG. 3. Comparison of the T. denticola fla promoter sequence with promoter sequences from various spirochete motility genes and consensus sigma 28 sequences.

The deduced amino acid sequence of T. denticola Tap1 was aligned with those of other known treponemal Tap1 homologs (Fig.4A). This alignment revealed extensive amino acid sequence identitywithin a 90-amino-acid region near the C terminus with less identityin the remainder of the polypeptide (Fig. 4A). The overall T.denticola Tap1 identity as determined with the GAP program was32% with T. phagedenis and 21% with T. pallidum. Within the conserved90-amino-acid region from F-324 to G-394, T. denticola has 30%amino acid sequence identity with FliK of S. typhimurium (16)as shown in Fig. 4B. BLAST 2.0 searches (2) with the 90-amino-acidconserved region also revealed a similar sequence identity withFliK proteins of Bacillus subtilis and Rhodobacter sphaeroides(references 1 and 11 and data not shown).

View larger version (62K):
[in this window]
[in a new window]

FIG. 4. Alignment of Tap1 amino acid sequences. (A) Identical amino acids from three treponemes are boxed and shaded with SHADYBOX, which reveals the conserved region near the carboxyl terminus. The dark inverted triangle indicates the location of the point of insertion for the erythromycin resistance cassette into the T. denticola tap1 gene to generate a Tap1-deficient mutant. (B) Alignment of the conserved C-terminal region of T. denticola Tap1 with FliK of S. typhimurium (16). Identical amino acids are boxed and shaded as described above.

Identification of a T. denticola flaB gene. PCR of T. denticola DNA with primers located in a conserved region of treponemal FlaB resulted in a 620-bp amplicon. Sequenceanalysis revealed the highest amino acid sequence identity (76%)with FlaB1 of T. pallidum. However, a definitive identity wasnot assigned to this T. denticola flaB gene because the 5' endof the gene was not sequenced. That sequence could have been usedfor comparison with the published N-terminal amino acid sequencesof T. denticola FlaB1, FlaB2, and FlaB3 (29). The T. denticolaflaB DNA sequence was essential for designing oligonucleotidesfor use in RT-PCR to determine whether a flaB gene was transcribed.Because of the extensive identity among flaB genes, we cannotexclude the possibility that the primers used in RT-PCR have amplifiedmore than one flaBgene.

Interruption of tap1 with antibiotic resistance cassettes. To create a specific mutant that was deficient in Tap1, a suicide plasmid that contained an ermF-ermAM cassette inserted withinT. denticola tap1 was constructed (Fig. 1 and 4A). Electroporation-mediatedallelic exchange replaced the wild-type tap1 with the interruptedversion in the T. denticola chromosome. Although the yields ofdouble-crossover recombinants are sometimes quite low (<10 coloniesper electroporation), this transformation with the ermF-ermAMcassette produced 533 colonies with linear DNA and 71 colonieswith uncut plasmid DNA after 1 week of incubation following electroporation.Although nonmethylated plasmid DNA was used for these transformations,we have subsequently found that E. coli-methylated DNA may alsobe used. Several colonies were selected for further analysis,but additional testing suggested that these were indistinguishableclones that had undergone a similar double-crossover recombinationevent to inactivate tap1 (data not shown). Therefore, one clonewas used for all subsequent analysis and is termed JS97. Southernblotting and PCR revealed that JS97 had incorporated the erythromycinresistance cassette within tap1 via double-crossover recombination(data notshown).

A second tap1-deficient mutant was generated with the modified ermF-ermAMnp cassette. This construct contained the ermF-ermAMnpcassette, which lacked the putative terminator and nonessentialDNA upstream of ermF. The transformation of T. denticola withthe ermF-ermAMnp cassette produced another mutant, termed AS98.As indicated below, there was no major difference in transcriptionbetween the T. denticola mutants containing ermF-ermAM or ermF-ermAMnpcassettes within tap1. Therefore, except as indicated, the datapresented below were obtained from the tap1 mutant containingthe original ermF-ermAM cassette (JS97). The MIC of erythromycinis at least 300 µg/ml for both JS97 andAS98.

Analysis of the Tap1-deficient mutant JS97 of T. denticola. (i) Colony and cell morphology and motility. The tap1 mutant JS97 produced greyish white raised colonies on 0.5% NOS-agarose with a colony diameter of 1 to 2 mm after7 days of incubation. There was no subsurface migration of JS97in agar plates even after 3 weeks of incubation (data not shown).In contrast, the wild-type colony spread beneath the agar surfaceto about 9 mm in diameter during this time. Figure 5 shows therelationship of spreading of the wild-type T. denticola to thatof JS97. In NOS broth, the tap1 mutant JS97 grew more slowly andto a lower density than the wild type (data not shown). Dark-fieldmicroscopic observations revealed that individual cells of JS97were generally longer than the wild type and tapered at the cellends (Fig. 6A). The cells exhibited no movement in liquid or viscousmedia. Electron microscopic analysis of the mutant JS97 showeda lack of flagellar filaments; however, the mutant did possesselongated flagellar hooks of variable length with a wavelike morphology(Fig. 6B, C, and D). To confirm the identity of the flagellarhooks, a cell lysate was enriched for hooks by a modificationof procedures described earlier (23). The final step of thisprocedure was to treat the samples with a low-pH (2.2) glycinebuffer, which disrupts flagellar filaments and basal bodies butleaves the flagellar hooks intact. As shown in Fig. 6C and D,electron microscopic analysis revealed that the long wavelikehooks remained after acid treatment, indicating that these structureswere not of flagellar filament origin. This sample reacted stronglyon immunoblots with antibodies raised against recombinant T. pallidumFlgE (data not shown and reference 23).

View larger version (143K):
[in this window]
[in a new window]

FIG. 5. T. denticola wild type (WT) and Tap1-deficient mutant JS97 after growth for 7 days on NOS plates containing 0.5% agarose. Approximately 0.1 µl was placed on the plate and incubated at 36°C in an anaerobic chamber.

View larger version (68K):
[in this window]
[in a new window]

FIG. 6. Microscopic analysis of the Tap1-deficient mutant JS97. (A) Dark-field micrograph. Bar, 5 µm. (B) Electron micrograph of a JS97 cell showing elongated hooks that do not possess flagellar filaments. The outer sheath was removed by treatment with 1% Triton X-100 reduced as indicated in the text. Bar, 100 nm. (C and D) Electron micrographs of preparations of enriched hooks from JS97. Bars, 100 nm.

(ii) Transcription analysis. RT-PCR was used to analyze transcription in the tap1 mutants containing ermF-ermAM (JS97) and ermF-ermAMnp (AS98). Becausethe tap1 gene is located in an operon, there was concern thatpotential polar effects from the ermF-ermAM cassette could resultin lack of transcription of all downstream genes. Previous studiessuggested that a putative transcription terminator was locatedbetween ermF and ermAM (6). By RT-PCR, transcription was analyzedupstream of the ermF-ermAM cassette (within tap1) and downstreamof the ermF-ermAM cassette (within flgD and flgE) (Fig. 1). Resultsindicate that transcription of these genes was not significantlyaltered and that the levels of RNA were comparable to those ofthe wild type (Fig. 7). In addition, flaB RNA was easily detectableby RT-PCR (Fig. 7) as were fliG, ermF, and ermAM RNA (data notshown).

View larger version (41K):
[in this window]
[in a new window]

FIG. 7. RT-PCR products after agarose gel electrophoresis and staining with ethidium bromide. W, wild-type T. denticola; A, Tap1-deficient mutant JS97; tap1, RT-PCR with primers 1 and 2 within tap1; tap1-flgD, RT-PCR with primers 3 and 4 downstream of the BglII site; flgE, RT-PCR with primers 5 and 6 (see Fig. 1 for the location of these primers); flaB, RT-PCR of the flagellar filament flaB gene with primers as described in Materials and Methods. Note that levels of RT-PCR products in the wild type and in JS97 are similar. Numbers at right are the molecular size markers in base pairs. Control reactions without RT did not show any bands (data not shown).

(iii) Protein expression determined by immunoblotting. Immunoblotting was done to assess expression of proteins within the fla operon (Tap1 and FlgE) and outside of the fla operon(FlaB) in the Tap1-deficient mutant. The T. denticola Tap1 antiserareacted with Tap1 (Fig. 8A) and also with at least one other polypeptide(data not shown) in wild-type T. denticola. The basis for thiscross-reaction is unknown. As shown in Fig. 8A, the Tap1-deficientmutants JS97 and AS98 produced no detectable level of Tap1. Incontrast, these mutants synthesized FlgE at approximately wild-typelevels (Fig. 8B). Surprisingly, the Tap1-deficient mutants expressedonly trace amounts of FlaB polypeptide compared to wild-type T.denticola (Fig. 8C). This result was unexpected because thesemutants possess a level of flaB RNA comparable to that of thewild type. Using immunoblotting, we determined that the flagellarsheath polypeptide, FlaA, was also present in only trace amounts(data not shown).

View larger version (19K):
[in this window]
[in a new window]

FIG. 8. Western blots with T. denticola Tap1 antiserum (A), T. pallidum FlgE antiserum (B), and T. phagedenis FlaB antiserum (C). Lanes 1, JS97; lanes 2, AS98; lanes 3, wild type. The arrow in panel A indicates the Tap1 polypeptide band. In panel B, the polypeptide ladder is a typical pattern found in treponemal hook polypeptides that may be due to cross-linking. The significance of the minor band missing in lane 3 is unknown. Numbers at right of each panel represent molecular masses in kilodaltons.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The genetic analysis of spirochetes has been hindered by the inability to generate specific mutations. In S. typhimurium andother better-defined systems, specific mutations have helped toascertain the function and regulation of genes involved in bacterialmotility. Although spirochetes and enteric bacteria have manyhomologs that are presumed to be involved in motility, the functionsin spirochetes are inferred from nucleotide and amino acid sequenceidentities. Comparative sequence analysis, although quite useful,has limitations for ascertaining the function of genes that haveno homologs in other bacteria. The recent discovery by Li et al.that an erythromycin resistance cassette could be used to inactivateT. denticola genes has proven to be a valuable tool for geneticmanipulation (19).

This work was designed primarily to identify, characterize, and then determine whether T. denticola tap1, a gene of unknownfunction, was essential for treponemal motility. T. denticolatap1 was identified as the first gene of the fla motility operon,an arrangement found in T. phagedenis and T. pallidum as well,which suggested a role of Tap1 in motility. Alignment of the aminoacid sequence of T. denticola Tap1 with other treponemal Tap1sequences revealed a well-conserved 90-amino-acid region nearthe C terminus and little identity in the remainder of the polypeptide.Moreover, the amino acid sequence of the conserved 90-amino-acidC-terminal region of T. denticola Tap1 possessed a modest identitywith FliK proteins of R. sphaeroides, B. subtilis, and S. typhimurium(1, 11, 16). These comparisons suggest that the C-terminalregion provides a fundamental conserved region necessary for thestructure or function of tap1. However, since there is limitedamino acid sequence identity to known genes, genetic evidencewas required to determine the role of Tap1 in T. denticolamotility.

Using the gene interruption technique of Li et al. (19), we specifically interrupted the carboxy-terminal region of T. denticolaTap1. The resulting mutant, JS97, was completely nonmotile andlacked periplasmic flagellar filaments but possessed flagellarhooks. Thus, genetic evidence showed that Tap1 was essential forT. denticola motility. Interestingly, these hooks were elongatedand of variable length compared with wild-type hooks. Our hypothesisis that Tap1 is involved in monitoring the length of the flagellarhook in T. denticola, a function that is performed by FliK inenteric bacteria (14, 16, 27, 34). It has been postulatedpreviously that the N terminus of FliK might function as a hooklength measurement domain and that the C terminus is responsiblefor flagellar export specificity in S. typhimurium (16). Frameshiftmutants disrupted in the C-terminal region of S. typhimurium FliKhave a hook length control defect together with a flagellar filament-negativephenotype (34). The variable hook length of T. denticola JS97together with a lack of flagellar filaments is similar to thephenotype of these FliK mutants of S. typhimurium (16, 34).Moreover, isolated hooks from JS97 clearly demonstrated variablelength, suggesting a lack of control on the hook length assembly.The morphology of these polyhooks is similar to that of knownFliK-deficient mutants of S. typhimurium (34). On the aminoacid level, the modest identity of the conserved C-terminal regionof Tap1 with S. typhimurium FliK suggests that these polypeptidesare homologs. Therefore, on the basis of the remarkable similarityof the phenotype of the Tap1-deficient T. denticola to that ofthe FliK mutants of S. typhimurium, we propose that Tap1 be designatedT. denticolaFliK.

One unexpected finding was that the Tap1 (FliK)-deficient mutant JS97 synthesized abundant levels of flaB flagellar filamentRNA and yet lacked flagellar filaments and FlaB polypeptides.Presumably, either the flagellar filament proteins are synthesizedand then rapidly degraded or there is an unknown form of translationalcontrol of filament protein synthesis. Enteric mutants with C-terminaldeletions of FliK also fail to assemble flagellar filaments (14,34); however, whether flagellar filament RNA is transcribedis not clear. This phenotype has been noted for other spirochetemotility mutants as well. For example, we reconstructed the T.denticola flgE mutant HL51 (29) and found wild-type levels offlaB RNA. However, HL51 does not possess flagellar filament structures(21, 29). In the FlgE-deficient mutant HL51, the lack of aflagellar hook structure should prevent the filament from assembling.In contrast to the FlgE mutant, the Tap1 (FliK)-deficient mutantJS97 synthesizes an intact hook structure, albeit one that isabnormally long; however, the flagellar filament may be unableto be assembled because the FliK deficiency renders the cell unableto switch to filament export (34). Both of these T. denticolamutants, HL51 and JS97, together with a previously described chemicallyderived mutant of T. phagedenis (20) and a spontaneous mutantof Borrelia burgdorferi (30) have a flagellar filament structure-deficientphenotype despite adequate filament RNA expression, suggestinga common spirochete response to mutations within certain motilitygenes. The basis for this unusual regulation of spirochete flagellarfilament protein synthesis isunknown.

The ermF-ermAM construct utilized by Li et al. possessed a putative transcription terminator (6). Consequently, we wereconcerned that the tap1 mutant JS97 was nonmotile because of polareffects on downstream genes. However, when the ermF-ermAM cassettewas analyzed with the TERMINATOR or RNAFOLD program in the Wisconsinpackage no significant transcription terminator was identified.To show that transcription was not terminated, we removed theputative terminator and some noncritical DNA to create a seconderythromycin resistance cassette. Both of these cassettes wereincorporated into T. denticola tap1 and showed similar levelsof fla operon RNA that were comparable to that of the wild type.Although quantitative RT-PCR or RNase protection studies werenot performed, it is clear that levels of RNA downstream of theermF-ermAM cassette were comparable to those of the wild typeand were sufficient for synthesis and assembly of flagellar componentssuch as FlgE. On the basis of the good transcription and translationof flgE in JS97, we believe that this cassette is useful for studyinggenes both within and outsideoperons.

In summary, using specific gene inactivation, we have shown that Tap1 is involved in the motility of T. denticola, perhapsby perturbation of the ability of the cell to monitor flagellarhook length or export. Various lines of evidence suggest thatTap1 performs a function analogous to that of FliK in other bacteria.Because the motility of spirochetes contributes to their pathogenesis,these studies could prove useful in creating specific avirulentor less-virulent strains as potential vaccinecandidates.

	ACKNOWLEDGMENTS

We acknowledge Mary Beth Kinoshita and Andrea Knaggs, Wadsworth Center Molecular Genetics and Electron Microscopy Core Facilities,Photography Unit, for technical assistance and Howard Kuramitsuand Hong Li for providing strains and advice on electroporationofspirochetes.

J.I. was supported in part by a basic research grant from Health Research Incorporated. This work was supported by PublicHealth Research Service grant AI34354 from the National InstitutesofHealth.

	FOOTNOTES

^* Corresponding author. Mailing address: David Axelrod Institute for Public Health, Wadsworth Center, New York State Departmentof Health, P.O. Box 22002, Albany, NY 12201-2002. Phone: (518)474-4177. Fax: (518) 486-7971. E-mail: Ron.Limberger{at}wadsworth.org.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Albertini, A. M., T. Caramori, W. D. Crabb, F. Scoffone, and A. Galizzi. 1991. The flaA locus of Bacillus subtilis is part of a large operon coding for flagellar structures, motility functions, and an ATPase-like polypeptide. J. Bacteriol. 173:3573-3579[Abstract/Free Full Text].

2. Altschul, S. F., T. L. Madden, A. A. Schaffer, J. Zhang, Z. Zhang, W. Miller, and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].

3. Charon, N. W., S. F. Goldstein, S. M. Block, K. Kurci, J. D. Ruby, J. A. Kreiling, and R. J. Limberger. 1992. Morphology and dynamics of protruding spirochete periplasmic flagella. J. Bacteriol. 174:832-840[Abstract/Free Full Text].

4. Compton, T. 1990. Degenerate primers for DNA amplification, p. 39-45. In M. A. Innis, D. H. Gelfand, J. J. Sninsky, and T. J. White (ed.), PCR protocols: a guide to methods and applications. Academic Press, Inc., New York, N.Y.

5. Dantuono, L. A. 1996. Characterization of the fla motility operon of Treponema phagedenis. M.S. thesis. State University of New York, Albany, N.Y.

6. Fletcher, H. M., H. A. Schenkein, R. M. Morgan, K. A. Bailey, C. R. Berry, and F. L. Macrina. 1995. Virulence of a Porphyromonas gingivalis W83 mutant defective in the prtH gene. Infect. Immun. 63:1521-1528[Abstract].

7. Fraser, C. M., S. Casjens, W. M. Huang, G. G. Sutton, R. Clayton, R. Lathigra, O. White, K. A. Ketchum, R. Dodson, E. K. Hickey, M. Gwinn, B. Dougherty, J. F. Tomb, R. D. Fleischmann, D. Richardson, J. Peterson, A. R. Kerlavage, J. Quackenbush, S. Salzberg, M. Hanson, R. van Vugt, N. Palmer, M. D. Adams, J. Gocayne, J. Weidman, T. Utterback, L. Watthey, L. McDonald, P. Artiach, C. Bowman, S. Garland, C. Fujii, M. Cotton, K. Horst, K. Roberts, B. Hatch, H. O. Smith, and J. C. Venter. 1997. Genomic sequence of a Lyme disease spirochaete, Borrelia burgdorferi. Nature 390:580-586[Medline].

8. Fraser, C. M., S. J. Norris, G. M. Weinstock, O. White, G. G. Sutton, R. Dodson, M. Gwinn, E. K. Hickey, R. Clayton, K. A. Ketchum, E. Sodergren, J. M. Hardham, M. P. McLeod, S. Salzberg, J. Peterson, H. Khalak, D. Richardson, J. K. Howell, M. Chidambaram, T. Utterback, L. McDonald, P. Artiach, C. Bowman, M. D. Cotton, C. Fujii, S. Garland, B. Hatch, K. Horst, K. Roberts, M. Sandusky, J. Weidman, H. O. Smith, and J. C. Venter. 1998. Complete genome sequence of Treponema pallidum, the syphilis spirochete. Science 281:375-388[Abstract/Free Full Text].

9. Ge, Y., and N. W. Charon. 1997. Molecular characterization of a flagellar/chemotaxis operon in the spirochete Borrelia burgdorferi. FEMS Microbiol. Lett. 153:425-431[Medline].

10. Ge, Y., I. G. Old, I. Saint Girons, and N. W. Charon. 1997. Molecular characterization of a large Borrelia burgdorferi motility operon which is initiated by a consensus $sigma$ ⁷⁰ promoter. J. Bacteriol. 179:2289-2299[Abstract/Free Full Text].

11. Gonzalez-Pedrajo, B., T. Ballado, A. Campos, R. E. Sockett, L. Camarena, and G. Dreyfus. 1997. Structural and genetic analysis of a mutant of Rhodobacter sphaeroides WS8 deficient in hook length control. J. Bacteriol. 179:6581-6588[Abstract/Free Full Text].

12. Hardham, J. M., J. G. Frye, and L. V. Stamm. 1995. Identification and sequences of the Treponema pallidum fliM', fliY, fliP, fliQ, fliR, and flhB' genes. Gene 166:57-64[Medline].

13. Heinzerling, H. F., M. Olivares, and R. A. Burne. 1997. Genetic and transcriptional analysis of flgB flagellar operon constituents in the oral spirochete Treponema denticola and their heterologous expression in enteric bacteria. Infect. Immun. 65:2041-2051[Abstract].

14. Hirano, T., S. Yamaguchi, K. Oosawa, and S. Aizawa. 1994. Roles of FliK and FlhB in determination of flagellar hook length in Salmonella typhimurium. J. Bacteriol. 176:5439-5449[Abstract/Free Full Text].

15. Holt, S. C. 1978. Anatomy and chemistry of spirochetes. Microbiol. Rev. 42:114-160[Free Full Text].

16. Kawagishi, I., M. Homma, A. W. Williams, and R. M. Macnab. 1996. Characterization of the flagellar hook length control protein fliK of Salmonella typhimurium and Escherichia coli. J. Bacteriol. 178:2954-2959[Abstract/Free Full Text].

17. Kimsey, R. B., and A. Spielman. 1990. Motility of Lyme disease spirochetes in fluids as viscous as the extracellular matrix. J. Infect. Dis. 162:1205-1208[Medline].

18. Klitorinos, A., P. Noble, R. Siboo, and E. C. Chan. 1993. Viscosity-dependent locomotion of oral spirochetes. Oral Microbiol. Immunol. 8:242-244[Medline].

19. Li, H., J. Ruby, N. Charon, and H. Kuramitsu. 1996. Gene inactivation in the oral spirochete Treponema denticola: construction of an flgE mutant. J. Bacteriol. 178:3664-3667[Abstract/Free Full Text].

20. Limberger, R. J., and N. W. Charon. 1986. Treponema phagedenis has at least two proteins residing together on its periplasmic flagella. J. Bacteriol. 166:105-112[Abstract/Free Full Text].

21. Limberger, R. J., and L. L. Slivienski. 1998. Unpublished observations.

22. Limberger, R. J., L. L. Slivienski, M. C. El-Afandi, and L. A. Dantuono. 1996. Organization, transcription, and expression of the 5' region of the fla operon of Treponema phagedenis and Treponema pallidum. J. Bacteriol. 178:4628-4634[Abstract/Free Full Text].

23. Limberger, R. J., L. L. Slivienski, and W. A. Samsonoff. 1994. Genetic and biochemical analysis of the flagellar hook of Treponema phagedenis. J. Bacteriol. 176:3631-3637[Abstract/Free Full Text].

24. Limberger, R. J., L. L. Slivienski, D. B. Yelton, and N. W. Charon. 1992. Molecular genetic analysis of a class B periplasmic flagellum gene of Treponema phagedenis. J. Bacteriol. 174:6404-6410[Abstract/Free Full Text].

25. Macnab, R. M. 1992. Genetics and biogenesis of bacterial flagella. Annu. Rev. Genet. 26:131-158[Medline].

26. Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

27. Muramoto, K., S. Makishima, S. I. Aizawa, and R. M. Macnab. 1998. Effect of cellular level of FliK on flagellar hook and filament assembly in Salmonella typhimurium. J. Mol. Biol. 277:871-882[Medline].

28. Ohnishi, K., Y. Ohto, S. Aizawa, R. M. Macnab, and T. Iino. 1994. FlgD is a scaffolding protein needed for flagellar hook assembly in Salmonella typhimurium. J. Bacteriol. 176:2272-2281[Abstract/Free Full Text].

29. Ruby, J. D., H. Li, H. Kuramitsu, S. J. Norris, S. F. Goldstein, K. F. Buttle, and N. W. Charon. 1997. Relationship of Treponema denticola periplasmic flagella to irregular cell morphology. J. Bacteriol. 179:1628-1635[Abstract/Free Full Text].

30. Sadziene, A., D. D. Thomas, V. G. Bundoc, S. C. Holt, and A. G. Barbour. 1991. A flagella-less mutant of Borrelia burgdorferi. Structural, molecular and in vitro functional characterization. J. Clin. Investig. 88:82-92.

31. Schleicher & Schuell.. 1987. Transfer and immobilization of nucleic acids to S&S solid supports. Schleicher & Schuell, Inc., Keene, N.H..

32. Simonson, L. G., C. H. Goodman, J. J. Bial, and H. E. Morton. 1988. Quantitative relationship of Treponema denticola to severity of periodontal disease. Infect. Immun. 56:726-728[Abstract/Free Full Text].

33. Smibert, R. M. 1984. Genus III. Treponema Schaudin 1905, 1728^AL, p. 49-57. In N. R. Krieg, and J. G. Holt (ed.), Bergey's manual of systematic bacteriology, vol. 1. The Williams and Wilkins Co., Baltimore, Md.

34. Williams, A. W., S. Yamaguchi, F. Togashi, S. I. Aizawa, I. Kawagishi, and R. M. Macnab. 1996. Mutations in fliK and flhB affecting flagellar hook and filament assembly in Salmonella typhimurium. J. Bacteriol. 178:2960-2970[Abstract/Free Full Text].

This article has been cited by other articles:

Yang, Y., Stewart, P. E., Shi, X., Li, C. (2008). Development of a Transposon Mutagenesis System in the Oral Spirochete Treponema denticola. Appl. Environ. Microbiol. 74: 6461-6464 [Abstract] [Full Text]
Sim, J.-H., Shi, W., Lux, R. (2005). Protein-protein interactions in the chemotaxis signalling pathway of Treponema denticola. Microbiology 151: 1801-1807 [Abstract] [Full Text]
Slivienski-Gebhardt, L. L., Izard, J., Samsonoff, W. A., Limberger, R. J. (2004). Development of a Novel Chloramphenicol Resistance Expression Plasmid Used for Genetic Complementation of a fliG Deletion Mutant in Treponema denticola. Infect. Immun. 72: 5493-5497 [Abstract] [Full Text]
Vesey, P. M., Kuramitsu, H. K. (2004). Genetic analysis of Treponema denticola ATCC 35405 biofilm formation. Microbiology 150: 2401-2407 [Abstract] [Full Text]
Motaleb, M. A., Sal, M. S., Charon, N. W. (2004). The Decrease in FlaA Observed in a flaB Mutant of Borrelia burgdorferi Occurs Posttranscriptionally. J. Bacteriol. 186: 3703-3711 [Abstract] [Full Text]
Lux, R., Sim, J.-H., Tsai, J. P., Shi, W. (2002). Construction and Characterization of a cheA Mutant of Treponema denticola. J. Bacteriol. 184: 3130-3134 [Abstract] [Full Text]
Chi, B., Limberger, R. J., Kuramitsu, H. K. (2002). Complementation of a Treponema denticola flgE Mutant with a Novel Coumermycin A1-Resistant T. denticola Shuttle Vector System. Infect. Immun. 70: 2233-2237 [Abstract] [Full Text]
Lux, R., Miller, J. N., Park, N.-H., Shi, W. (2001). Motility and Chemotaxis in Tissue Penetration of Oral Epithelial Cell Layers by Treponema denticola. Infect. Immun. 69: 6276-6283 [Abstract] [Full Text]
Xu, X., Holt, S. C., Kolodrubetz, D. (2001). Cloning and Expression of Two Novel Hemin Binding Protein Genes from Treponema denticola. Infect. Immun. 69: 4465-4472 [Abstract] [Full Text]
Izard, J., Samsonoff, W. A., Limberger, R. J. (2001). Cytoplasmic Filament-Deficient Mutant of Treponema denticola Has Pleiotropic Defects. J. Bacteriol. 183: 1078-1084 [Abstract] [Full Text]
Sela, M. N. (2001). Role of Treponema Denticola in Periodontal Diseases. CROBM 12: 399-413 [Abstract] [Full Text]
Motaleb, M. A., Corum, L., Bono, J. L., Elias, A. F., Rosa, P., Samuels, D. S., Charon, N. W. (2000). Borrelia burgdorferi periplasmic flagella have both skeletal and motility functions. Proc. Natl. Acad. Sci. USA 10.1073/pnas.200221797v1 [Abstract] [Full Text]
Izard, J., Samsonoff, W. A., Kinoshita, M. B., Limberger, R. J. (1999). Genetic and Structural Analyses of Cytoplasmic Filaments of Wild-Type Treponema phagedenis and a Flagellar Filament-Deficient Mutant. J. Bacteriol. 181: 6739-6746 [Abstract] [Full Text]
Motaleb, M. A., Corum, L., Bono, J. L., Elias, A. F., Rosa, P., Samuels, D. S., Charon, N. W. (2000). Borrelia burgdorferi periplasmic flagella have both skeletal and motility functions. Proc. Natl. Acad. Sci. USA 97: 10899-10904 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Limberger, R. J.
	Articles by Samsonoff, W. A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Limberger, R. J.
	Articles by Samsonoff, W. A.

1.	Albertini, A. M., T. Caramori, W. D. Crabb, F. Scoffone, and A. Galizzi. 1991. The flaA locus of Bacillus subtilis is part of a large operon coding for flagellar structures, motility functions, and an ATPase-like polypeptide. J. Bacteriol. 173:3573-3579[Abstract/Free Full Text].
2.	Altschul, S. F., T. L. Madden, A. A. Schaffer, J. Zhang, Z. Zhang, W. Miller, and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].
3.	Charon, N. W., S. F. Goldstein, S. M. Block, K. Kurci, J. D. Ruby, J. A. Kreiling, and R. J. Limberger. 1992. Morphology and dynamics of protruding spirochete periplasmic flagella. J. Bacteriol. 174:832-840[Abstract/Free Full Text].
4.	Compton, T. 1990. Degenerate primers for DNA amplification, p. 39-45. In M. A. Innis, D. H. Gelfand, J. J. Sninsky, and T. J. White (ed.), PCR protocols: a guide to methods and applications. Academic Press, Inc., New York, N.Y.
5.	Dantuono, L. A. 1996. Characterization of the fla motility operon of Treponema phagedenis. M.S. thesis. State University of New York, Albany, N.Y.
6.	Fletcher, H. M., H. A. Schenkein, R. M. Morgan, K. A. Bailey, C. R. Berry, and F. L. Macrina. 1995. Virulence of a Porphyromonas gingivalis W83 mutant defective in the prtH gene. Infect. Immun. 63:1521-1528[Abstract].
7.	Fraser, C. M., S. Casjens, W. M. Huang, G. G. Sutton, R. Clayton, R. Lathigra, O. White, K. A. Ketchum, R. Dodson, E. K. Hickey, M. Gwinn, B. Dougherty, J. F. Tomb, R. D. Fleischmann, D. Richardson, J. Peterson, A. R. Kerlavage, J. Quackenbush, S. Salzberg, M. Hanson, R. van Vugt, N. Palmer, M. D. Adams, J. Gocayne, J. Weidman, T. Utterback, L. Watthey, L. McDonald, P. Artiach, C. Bowman, S. Garland, C. Fujii, M. Cotton, K. Horst, K. Roberts, B. Hatch, H. O. Smith, and J. C. Venter. 1997. Genomic sequence of a Lyme disease spirochaete, Borrelia burgdorferi. Nature 390:580-586[Medline].
8.	Fraser, C. M., S. J. Norris, G. M. Weinstock, O. White, G. G. Sutton, R. Dodson, M. Gwinn, E. K. Hickey, R. Clayton, K. A. Ketchum, E. Sodergren, J. M. Hardham, M. P. McLeod, S. Salzberg, J. Peterson, H. Khalak, D. Richardson, J. K. Howell, M. Chidambaram, T. Utterback, L. McDonald, P. Artiach, C. Bowman, M. D. Cotton, C. Fujii, S. Garland, B. Hatch, K. Horst, K. Roberts, M. Sandusky, J. Weidman, H. O. Smith, and J. C. Venter. 1998. Complete genome sequence of Treponema pallidum, the syphilis spirochete. Science 281:375-388[Abstract/Free Full Text].
9.	Ge, Y., and N. W. Charon. 1997. Molecular characterization of a flagellar/chemotaxis operon in the spirochete Borrelia burgdorferi. FEMS Microbiol. Lett. 153:425-431[Medline].
10.	Ge, Y., I. G. Old, I. Saint Girons, and N. W. Charon. 1997. Molecular characterization of a large Borrelia burgdorferi motility operon which is initiated by a consensus $sigma$ ⁷⁰ promoter. J. Bacteriol. 179:2289-2299[Abstract/Free Full Text].
11.	Gonzalez-Pedrajo, B., T. Ballado, A. Campos, R. E. Sockett, L. Camarena, and G. Dreyfus. 1997. Structural and genetic analysis of a mutant of Rhodobacter sphaeroides WS8 deficient in hook length control. J. Bacteriol. 179:6581-6588[Abstract/Free Full Text].
12.	Hardham, J. M., J. G. Frye, and L. V. Stamm. 1995. Identification and sequences of the Treponema pallidum fliM', fliY, fliP, fliQ, fliR, and flhB' genes. Gene 166:57-64[Medline].
13.	Heinzerling, H. F., M. Olivares, and R. A. Burne. 1997. Genetic and transcriptional analysis of flgB flagellar operon constituents in the oral spirochete Treponema denticola and their heterologous expression in enteric bacteria. Infect. Immun. 65:2041-2051[Abstract].
14.	Hirano, T., S. Yamaguchi, K. Oosawa, and S. Aizawa. 1994. Roles of FliK and FlhB in determination of flagellar hook length in Salmonella typhimurium. J. Bacteriol. 176:5439-5449[Abstract/Free Full Text].
15.	Holt, S. C. 1978. Anatomy and chemistry of spirochetes. Microbiol. Rev. 42:114-160[Free Full Text].
16.	Kawagishi, I., M. Homma, A. W. Williams, and R. M. Macnab. 1996. Characterization of the flagellar hook length control protein fliK of Salmonella typhimurium and Escherichia coli. J. Bacteriol. 178:2954-2959[Abstract/Free Full Text].
17.	Kimsey, R. B., and A. Spielman. 1990. Motility of Lyme disease spirochetes in fluids as viscous as the extracellular matrix. J. Infect. Dis. 162:1205-1208[Medline].
18.	Klitorinos, A., P. Noble, R. Siboo, and E. C. Chan. 1993. Viscosity-dependent locomotion of oral spirochetes. Oral Microbiol. Immunol. 8:242-244[Medline].
19.	Li, H., J. Ruby, N. Charon, and H. Kuramitsu. 1996. Gene inactivation in the oral spirochete Treponema denticola: construction of an flgE mutant. J. Bacteriol. 178:3664-3667[Abstract/Free Full Text].
20.	Limberger, R. J., and N. W. Charon. 1986. Treponema phagedenis has at least two proteins residing together on its periplasmic flagella. J. Bacteriol. 166:105-112[Abstract/Free Full Text].
21.	Limberger, R. J., and L. L. Slivienski. 1998. Unpublished observations.
22.	Limberger, R. J., L. L. Slivienski, M. C. El-Afandi, and L. A. Dantuono. 1996. Organization, transcription, and expression of the 5' region of the fla operon of Treponema phagedenis and Treponema pallidum. J. Bacteriol. 178:4628-4634[Abstract/Free Full Text].
23.	Limberger, R. J., L. L. Slivienski, and W. A. Samsonoff. 1994. Genetic and biochemical analysis of the flagellar hook of Treponema phagedenis. J. Bacteriol. 176:3631-3637[Abstract/Free Full Text].
24.	Limberger, R. J., L. L. Slivienski, D. B. Yelton, and N. W. Charon. 1992. Molecular genetic analysis of a class B periplasmic flagellum gene of Treponema phagedenis. J. Bacteriol. 174:6404-6410[Abstract/Free Full Text].
25.	Macnab, R. M. 1992. Genetics and biogenesis of bacterial flagella. Annu. Rev. Genet. 26:131-158[Medline].
26.	Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
27.	Muramoto, K., S. Makishima, S. I. Aizawa, and R. M. Macnab. 1998. Effect of cellular level of FliK on flagellar hook and filament assembly in Salmonella typhimurium. J. Mol. Biol. 277:871-882[Medline].
28.	Ohnishi, K., Y. Ohto, S. Aizawa, R. M. Macnab, and T. Iino. 1994. FlgD is a scaffolding protein needed for flagellar hook assembly in Salmonella typhimurium. J. Bacteriol. 176:2272-2281[Abstract/Free Full Text].
29.	Ruby, J. D., H. Li, H. Kuramitsu, S. J. Norris, S. F. Goldstein, K. F. Buttle, and N. W. Charon. 1997. Relationship of Treponema denticola periplasmic flagella to irregular cell morphology. J. Bacteriol. 179:1628-1635[Abstract/Free Full Text].
30.	Sadziene, A., D. D. Thomas, V. G. Bundoc, S. C. Holt, and A. G. Barbour. 1991. A flagella-less mutant of Borrelia burgdorferi. Structural, molecular and in vitro functional characterization. J. Clin. Investig. 88:82-92.
31.	Schleicher & Schuell.. 1987. Transfer and immobilization of nucleic acids to S&S solid supports. Schleicher & Schuell, Inc., Keene, N.H..
32.	Simonson, L. G., C. H. Goodman, J. J. Bial, and H. E. Morton. 1988. Quantitative relationship of Treponema denticola to severity of periodontal disease. Infect. Immun. 56:726-728[Abstract/Free Full Text].
33.	Smibert, R. M. 1984. Genus III. Treponema Schaudin 1905, 1728^AL, p. 49-57. In N. R. Krieg, and J. G. Holt (ed.), Bergey's manual of systematic bacteriology, vol. 1. The Williams and Wilkins Co., Baltimore, Md.
34.	Williams, A. W., S. Yamaguchi, F. Togashi, S. I. Aizawa, I. Kawagishi, and R. M. Macnab. 1996. Mutations in fliK and flhB affecting flagellar hook and filament assembly in Salmonella typhimurium. J. Bacteriol. 178:2960-2970[Abstract/Free Full Text].