The Bacteroides fragilis BtgA Mobilization Protein Binds to the oriT Region of pBFTM10

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Journal of Bacteriology, September 1998, p. 4922-4928, Vol. 180, No. 18
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

The Bacteroides fragilis BtgA Mobilization Protein Binds to the oriT Region of pBFTM10

Leonid A. Sitailo,¹ Alexander M. Zagariya,¹^, Patrick J. Arnold,¹ Gayatri Vedantam,¹ and David W. Hecht¹^,²^,^*

Department of Medicine, VA Hospital, Hines, Illinois 60141,¹ and Department of Medicine, Microbiology and Immunology, Program in Molecular Biology, Loyola University Chicago, Maywood, Illinois 60153²

Received 15 January 1998/Accepted 13 July 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The Bacteroides fragilis conjugal plasmid pBFTM10 contains two genes, btgA and btgB, and a putative oriT region necessaryfor transfer in Bacteroides fragilis and Escherichia coli. TheBtgA protein was predicted to contain a helix-turn-helix motif,indicating possible DNA binding activity. DNA sequence analysisof the region immediately upstream of btgA revealed three setsof inverted repeats, potentially locating the oriT region. A 304-bpDNA fragment comprising this putative oriT region was cloned andconfirmed to be the functional pBFTM10 oriT by bacterial conjugationexperiments using E. coli and B. fragilis. btgA was cloned andoverexpressed in E. coli, and the purified protein was used inelectrophoretic mobility shift assays, demonstrating specificbinding of BtgA protein to its cognate oriT. DNase I footprintanalysis demonstrated that BtgA binds apparently in a single-strandedfashion to the oriT-containing fragment, overlapping invertedrepeats I, II, and III and the putative nick site.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial conjugation is a major mechanism for the transfer of chromosomal or plasmid DNA between prokaryotic cells. As aresult, dissemination of antibiotic resistance determinants canoccur, significantly influencing the virulence of various pathogenssuch as Escherichia coli, agrobacteria, enterococci, staphylococci,streptococci, streptomycetes, and the Bacteroides fragilis group(2, 4, 10, 22, 33, 34). The initial reactions duringconjugal DNA transfer require multiple complex protein-DNA andprotein-protein interactions that result in the formation of arelaxosome at the cis-acting origin of transfer (oriT). Relaxosomesare stable nucleoprotein complexes resulting in site- and strand-specificnicking at a site (the nic site) in the oriT region (24). Therelaxase, or DNA strand transferase, cleaves at this nic siteand attaches covalently to the 5' terminus. DNA is transmittedunidirectionally as a single strand into a recipient cell with5'-to-3' polarity in a rolling-circle manner, followed by complementary-strandsynthesis in the new host (for detailed reviews of conjugativetransfer involving R and F factors, see references 25 and 44).

Much attention has been focused on the biochemical processes involved in the initiation of DNA transfer of the IncP $alpha$ plasmidRP4. The generation of the single DNA strand that is transferredrequires formation of the initiation complex, or DNA relaxosome,in a cascade-like fashion. The first step in relaxosome formationis binding of an RP4 protein, TraJ, to a 19-bp inverted repeatwithin the oriT region and a 10-bp palindrome, srj (24, 43).In the second step, TraI, another RP4 protein, binds TraJ by bothprotein-protein interactions and the recognition of a 6-bp sequence,sri, in the nic region. Subsequently, site- and strand-specificcleavage of a unique phosphodiester bond at the nic site of thetransfer origin occurs, followed by covalent attachment of TraIto the 5' terminus of the DNA strand involved in transfer. Thebinding and nicking events are thought to be independent processes(16, 26). TraI is also able to induce a second cleavage reactionproposed to terminate the rolling-circle model of transfer DNAreplication (27). Following strand transfer to a new host, TraIcatalyzes the recombination of two single-stranded DNA moleculesat the RP4 nic site (27). A third protein, TraH, stabilizesthe TraJ and TraI nucleoprotein complex by specific protein-proteininteractions and does not bind DNA itself (24, 45). A fourthprotein, TraK, interacts with oriT by binding DNA as a tetramerover a range of approximately 180 nucleotides, downstream of nic(46). Binding of TraK increases the formation of relaxationcomplexes in vitro and in vivo, possibly by influencing DNA topologyto expose the nic site for more efficient cleavage by TraI (43).

Transferable antibiotic resistance plasmids of the B. fragilis group have also been described. They include the clindamycin-resistantplasmids pBFTM10 (12), pBF4 (40), and pBI136 (31) and themetronidazole-resistant plasmids pIP417, pIP419, and pIP421 (11,37, 38). pBFTM10 is a 14.9-kb plasmid that is transferablewithin B. fragilis. When pBFTM10 is fused to the E. coli repliconpDG5 to form pGAT400, it can also transfer from B. fragilis toE. coli. Further, pGAT400 is also mobilizable within E. coli whencoresident with the IncP $beta$ plasmid R751, but it requires an intactpBFTM10 transfer region (12). Characterization of the pBFTM10transfer region has demonstrated that only two genes, btgA andbtgB, are necessary for transfer within B. fragilis and mobilizationby R751 in E. coli. DNA sequence analysis of btgA revealed a helix-turn-helixDNA binding motif, suggesting that it was a DNA binding protein(12). In addition, the identification of three sets of invertedrepeats (IRI, IRII, and IRIII) and a putative nic site in theregion upstream of btgA suggested that this was the pBFTM10 oriT(12, 39).

In this paper, we report the cloning of the pBFTM10 oriT and the expression and purification of the BtgA protein, and we demonstratespecific binding of BtgA to its cognate oriT as determined bymobility shift assays and footprinting analyses.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and media. The bacterial strains and plasmids used in this study are listed in Table 1. Media, antibiotic concentrations, and E. coligrowth conditions were as previously described (1, 20). BactoAgar and tryptone were obtained from Difco Co. (Detroit, Mich.).For strains requiring antibiotic selection, cells were grown at37°C overnight in Luria broth (LB) supplemented with 200 µg ofampicillin per ml. E. coli XL1-Blue was used for routine cloningprocedures (29). The putative oriT region was cloned into theBamHI site of pGEM-7Zf(+) (Promega, Madison, Wis.), to give pGEM-7ZT,and into the BamHI site of pACYC184, to form pJAYC1. E. coli BL21(DE3)was used as the host for btgA cloning and protein expression.A 646-bp fragment containing btgA was cloned into the BamHI siteof the expression vector pET-19b (Novagen, Madison, Wis.) to givepDHBA.

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TABLE 1. E. coli strains and plasmids

Plasmid mobilization experiments. All mating experiments were performed as previously described (12, 23), in triplicate, using E. coli HB101 cells containingR751 as donors and E. coli DW1030 cells as recipients (Table 1).Bacterial cultures were grown overnight at 37°C in LB with theappropriate antibiotics. Overnight cultures were diluted 10-foldin LB and grown to early log phase. In a sterile microcentrifugetube, 0.15 ml of donor cells was mixed with 1.35 ml of DW1030cells and then pelleted by centrifugation at 10,000 × g for 1min. After the supernatant was discarded, cell pellets were resuspendedin 100 µl of 1× MPBS (8 mM Na₂HPO₄, 2 mM NaH₂PO₄, 145 mM NaCl[pH 6.9]). Resuspended cells were then spotted onto sterile 25-mm,0.45-µm-pore-size Gelman GN-6 cellulose nitrate filters (NalgeCo., Rochester, N.Y.) on Luria agar plates and incubated at 37°Cfor 180 min. Transconjugants were enumerated by plating on selectivemedia, and the mobilization frequencies of plasmids were normalizedto the number of R751 transconjugants from the same experiment.The mobilization frequency of R751 was calculated as the mean± standard error of the number of R751 transconjugants dividedby the number of viable R751 donor cells.

DNA manipulations and enzymes. General DNA techniques were performed as described by Ausubel et al. (1). Purification of DNA for cloning was accomplishedby using Geneclean II (Bio 101 Inc., Vista, Calif.) as recommendedby the manufacturer. Competent E. coli BL21(DE3) cells for transformationwere prepared by the calcium chloride method (3). Restrictionendonucleases, T4 polynucleotide kinase, and pGEM-7Zf(+) wereobtained from Promega, MunI was obtained from Boehringer Mannheim(Indianapolis, Ind.), and DNase I was obtained from WorthingtonCo. (Freehold, N.J.).

PCR techniques. The GeneAmp core reagent kit (Perkin-Elmer Cetus Co., Norwalk, Conn.) was used according to the manufacturer's specificationsfor all PCR amplifications, which were performed on a Perkin-ElmerCetus GeneAmp PCR System 2400 thermal cycler with plasmid pGAT400(12) as the template. Two primers, arot5B (5'-GGTGTAGTGGGATCCAGGTTCTTTCTTAGTGCC-3')and arot3B (5'-CGCGGATCCGACAGAAGTGGTTGTTTC-3'), were used to introduceBamHI restriction endonuclease sites at both ends of the oriTregion cloned into the pGEM-7Zf(+) (Fig. 1) to give pJA-7ZT. Primerarot5B is complementary to nucleotides 334 to 351 upstream ofthe inverted repeats, and primer arot3B is complementary to nucleotides621 through 638 immediately downstream of the inverted repeats(12). Similarly, primers arba5N (5'-CGCGGATCCTATGGATAAAGAAACAACAACC-3')and arba3B (5'-CGATGGATCCTACCGCCTCCCTGTATCTTAC-3') were used tointroduce a BamHI restriction endonuclease site at the 5' and3' ends of the B. fragilis btgA gene for cloning in pET-19b/BamHIto give pDHBA. All PCR products were electrophoresed through 1.3%agarose gels. The appropriate bands (646 bp for btgA and 304 bpfor the oriT region) were excised and purified by using GenecleanII (Bio 101) prior to restriction endonuclease treatment and cloning.

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FIG. 1. Schematic representation of the pBFTM10 transfer region. Base pair numbers correspond to those used by Hecht et al. (12). Open rectangles represent the positions of the DNA oligonucleotides used for PCR amplification of the oriT region and the btgA gene: a, arba5N; b, arba3B; c, arot5B; and d, arot3B. The expanded view of the oriT region illustrates the positions of IRI, IRII, and IRIII relative to the start codon (ATG) of the btgA gene.

DNA sequence determination. Sequencing was performed by the Sanger dideoxy-chain termination method, using a Sequenase version 2.0 reagent kit as specifiedby the manufacturer (Amersham Co., Arlington Heights, Ill.).

Protein expression and purification. The BtgA protein was purified by an affinity binding procedure using His-Tag resin as specified by the manufacturer (Novagen).In brief, an overnight culture of E. coli BL21(DE3) carrying pDHBAwas diluted 10-fold in fresh LB with ampicillin at a final concentrationof 200 µg/ml and incubated at 37°C. Isopropyl- $beta$ -D-thiogalactopyranoside(IPTG) was then added to a final concentration of 1.0 mM, andcells were grown at 37°C with aeration for another 2 h beforeharvesting. Harvested cells were kept on ice and lysed by sonicdisruption in a binding buffer containing 5 mM imidazole, 0.5M NaCl, and 20 mM Tris-HCl (pH 7.9). Cell debris was removed bycentrifugation at 4°C at 10,000 × g and cell extracts were incubatedwith His-Tag resin for 30 min at 4°C with gentle rotation.

BtgA was eluted from the His-Tag resin in buffer containing 400 mM imidazole, 6 M urea, 0.5 M NaCl, and 20 mM Tris-HCl (pH7.9). Single-step dialysis to native conditions in storage buffer(20 mM Tris-HCl, 100 mM NaCl, 10 mM $beta$ -mercaptoethanol, 0.5 mMEDTA, 15% glycerol [pH 7.9]) yielded mostly insoluble protein.Therefore, the following dialysis steps were carried out to reducethe urea, salt, and imidazole concentrations: the first dialysis,to 100 mM imidazole, 2 M urea, and 200 mM NaCl; the second, to10 mM imidazole, 0.5 M urea, and 100 mM NaCl; the third, to 100mM urea and 100 mM NaCl; and the fourth, to storage buffer (20mM Tris-HCl [pH 7.9], 100 mM NaCl, 10 mM $beta$ -mercaptoethanol, 0.1mM EDTA, 15% glycerol). With this method, approximately 85% ofpurified protein was recovered in soluble form. The protein concentrationwas determined with the Bradford reagent (Bio-Rad Co., Hercules,Calif.), aliquoted, and stored at $-$ 80°C. Aliquots of BtgA weremixed with an equal volume of 2× sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) sample buffer, boiled for 5 min,and subjected to SDS-PAGE on 10% gels (15). Gels were stainedwith 0.5% Coomassie brilliant blue (Boehringer Mannheim) in 25%methanol-10% acetic acid.

Protein sequencing. An overnight culture of E. coli BL21(DE3) carrying pDHBA was grown under the conditions described above for protein expression.After IPTG induction, final harvesting, and resuspension in water,100 µl of whole cells was mixed with 100 µl of 2× SDS-PAGE samplebuffer (15) and boiled for 5 min. An aliquot was then applieddirectly to an SDS-10% polyacrylamide gel and electrophoresedat 100 V for 1 h. Proteins from the gel were transferred to aProBlott membrane according to the manufacturer's instructions.After Ponceau-S (Sigma) protein staining, the BtgA protein bandwas excised and sequenced. The first 24 amino-terminal amino acidswere sequenced with an ABI 477A protein sequencer (Applied BiosystemsCo., Foster, Calif.) with an on-line ABI 120A phenylthiohydantoinanalyzer. This analysis confirmed the correct fusion between thevector and BtgA protein.

DNA labeling and DNA mobility shift assay. The 304-bp oriT fragment was obtained by excision from pGEM-7ZT via BamHI restriction or by PCR. The resulting 304-bp oriTfragment was isolated by electrophoresis through a 1.3% agarosegel, purified by using Geneclean II, and labeled for footprintingassays using T4 DNA polynucleotide kinase as described by Sambrooket al. (29), with some modifications. When BamHI digestion wasused, a dephosphorylation step was included. The labeling mixcontained the 5' terminus of dephosphorylated DNA (1 to 50 pmol),10× bacteriophage T4 polynucleotide kinase buffer (5 µl), [ $gamma$ -³²P]ATP (3,000 Ci/mmol; 10 mCi/ml; 5 µl; Amersham Co., ArlingtonHeights, Ill.), bacteriophage T4 polynucleotide kinase (10 U),and water to 50 µl. If a higher efficiency of labeling was required,the reaction was performed in a volume of 20 µl, using 10 µCiof [ $gamma$ -³²P]ATP (3,000 Ci/mmol; 10 mCi/ml). After incubation of this mixturefor 30 min at 37°C, the enzyme was heat inactivated at 95°C for5 min (29). Labeled fragments were then subjected to restrictionendonuclease cleavage (with MunI, to obtain a 271-bp double-strandedDNA fragment specifically labeled on the upper strand, and withDdeI, to obtain a 295-bp double-stranded DNA fragment specificallylabeled on the lower strand) overnight at 37°C. Labeled fragmentswere purified by electrophoresis through a 5% acrylamide-0.5×Tris-borate-EDTA gel. The purified DNA band was visualized byautoradiography, excised, eluted overnight with water, and usedin DNase I footprinting assays.

For electrophoretic mobility shift assays, the 304-bp oriT fragment was labeled by using T4 polynucleotide kinase as describedabove, but with no subsequent restriction. The labeled fragmentwas purified from unincorporated nucleotides by acrylamide-gelelectrophoresis followed by elution. DNA binding reactions wereperformed in a 40-µl final volume of the binding buffer [10 mMTris-HCl (pH 7.9), 5 mM MgCl₂, 1 mM CaCl₂, 100 mM KCl, 2 mM dithiothreitol,50 µg of bovine serum albumin per ml, 2 µg of sonicated calf thymusDNA per ml, 1 µg of poly(dI-dC) (Boehringer Mannheim)] (1).Samples were incubated at room temperature for 30 min; then anequal volume of stop solution containing glycerol (final concentration,5%) and bromophenol blue (1 mg/ml) was added prior to loadingonto a 5% native acrylamide-0.5× Tris-borate-EDTA gel. Gels wereprerun for 1 h, or until the current had stabilized, with bufferin the upper tank replaced with fresh buffer before loading thesamples. Electrophoresis was started at 100 V and, after 10 min,changed to a constant voltage of 200 V at 4°C for 2 h. Gels werevacuum dried and exposed to Kodak X-Omat AR-5 film.

DNase I footprinting. DNase I footprinting analysis was performed as described by Galas and Schmitz (8). Briefly, 10 ng of the oriT fragment(specifically labeled on the upper or lower strand) was incubatedfor 30 min at 4°C with various concentrations of purified BtgAprotein in 1× binding buffer used for the gel shift assay describedabove, in a total reaction mixture volume of 40 µl. An equal volumeof the mixture (40 µl) containing 2 mM CaCl₂ and 15 mM MgCl₂ wasadded, and the cleavage reaction was carried out in a total volumeof 80 µl by adding DNase I to 2 ng. After 1 min of incubationat room temperature, DNase I was inactivated by adding an equalvolume (80 µl) of stop solution containing 10 mM EDTA, 0.5% SDS,100 mM NaCl, and 75 mg of tRNA per ml. Following phenol extractionand ethanol precipitation, samples were washed with 70% ethanol,dissolved in formamide dye solution, electrophoresed on an 8%polyacrylamide sequencing gel (28), and visualized by autoradiography.To resolve longer nucleotide sequences, increased electrophoresistime and Long Ranger acrylamide (FMC Bioproducts, Rockland, Maine)were used.

Digital imaging and data presentation. Autoradiographs and Coomassie blue-stained gels were scanned with a ScanMaker III (Microtek, Palm Bay, Fla.) or Hewlett-PackardScanJet 4C (Hewlett-Packard, Louisville, Ky.) flatbed scannerat high resolution (1,000 dots/inch), using the software applicationAdobe Photoshop version 3.0.5 (Adobe Systems Inc., Buffalo, N.Y.).Scanned images were then transferred to the application MicrosoftPowerpoint 4.0, text and labels were added, and images were printedat high resolution (1,440 dots/inch) on an Epson Stylus Color1520 printer (Epson America Inc., Torrance, Calif.). Hewlett-Packardsatin-gloss heavy-weight photographic paper was used for all prints.

Nucleotide sequence accession number. The GenBank accession number for the pBFTM10 mobilization region is M77806.

	RESULTS

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Cloning the oriT region of pBFTM10. Previous DNA sequence analysis of the pBFTM10 mobilization region in pGAT400 revealed three sets of inverted repeats and apossible nic site, based on consensus sequence immediately upstreamof btgA (12). In addition, preliminary DNA relaxosome isolationstudies also demonstrated that single-stranded DNA nicking occurredin or near this region (unpublished data). To determine if thisarea served as a functional oriT and a likely binding region forbtgA, a 304-bp fragment encompassing the three inverted repeatsand the putative nic site was initially amplified by PCR usingplasmid pGAT400 as a template. Figure 1 illustrates the transferregion of pBFTM10 and the locations of the PCR primers (see Materialsand Methods). Following cloning into the pGEM-7Zf(+) BamHI site,DNA sequence analysis confirmed that the amplified oriT regionwas properly cloned without any PCR-induced errors. The 304-bporiT fragment was then excised, cloned again into the unique BamHIsite of pACYC184 to form pJAYC1, and used in bacterial conjugationexperiments.

Demonstration of oriT function by bacterial conjugation. Previously, pGAT400 was shown to mobilize between E. coli mating pairs when coresident with R751. pGAT400 contains btgA andbtgB, both necessary for its own transfer, while R751 is presumedto provide the machinery necessary for transfer between E. colicells (12, 17, 19, 30). To determine if the cloned putativeoriT region was functional, pJAYC1 was transformed into E. coliHB101 containing pGAT400 and R751, or R751 alone, and used asa donor in bacterial conjugation experiments. HB101 cells containingeither pGAT400, R751, pJAYC1, or pACYC184 were used as negativecontrols.

Donor cells containing pGAT400 and R751 together with either pJAYC1 or pACYC184 were mixed with E. coli recipient DW1030 inmating experiments, and the transfer frequencies of R751, pGAT400,pJAYC1, and pACYC184 were determined. Throughout all mating experiments,the transfer frequencies of R751 ([1.87 ± 0.23] × 10²) and pGAT400 ([5.72 ± 0.64] × 10²; normalized to the level for R751) were similar to previouslyobserved values (12). When coresident with both pGAT400 andR751, pJAYC1 was mobilized to DW1030 at a frequency of (4.29 ±1.18) × 10² (normalized to the level for R751), similar to that of pGAT400.However, when coresident with R751 alone or when present withno coresident plasmid, pJAYC1 was not mobilized, indicating therequirement for pGAT400. In addition, when the donor harboredpJAYC1 and pGAT400 in the absence of R751, pJAYC1 was not mobilized,indicating the requirement for R751 for mobilization in E. coli.As expected, pACYC184 did not mobilize when coresident with eitherR751 or pGAT400 or with both.

To ensure that pJAYC1 transfer was not the result of cointegrate formation with pGAT400, transconjugants were plated on selectivemedia and assayed for cotransfer of pGAT400 and pJAYC1 (see Materialsand Methods). Only 15% of 200 Sp^r Cm^r pJAYC1 transconjugants contained pGAT400 (Amp^r), while only 1% of 100 Sp^r Amp^r pGAT400 transconjugants contained pJAYC1 (Cm^r). Restriction endonuclease treatment of plasmid DNA isolatedfrom 20 Sp^r Cm^r Amp^s or Sp^r Cm^r Amp^r pJAYC1 transconjugants confirmed that pJAYC1 and pGAT400 werenot altered, and cointegration of pJAYC1 with either pGAT400 orR751 did not occur (data not shown). In addition, R751 was foundin 100% of pGAT400 transconjugants but only 85% of pJAYC1 transconjugants.These findings indicated that pGAT400 and pJAYC1 cotransfer wasrare and not the result of cointegrate formation. Thus, the 304-bppBFTM10 DNA fragment cloned in pJAYC1 contained a functional oriT,and pJAYC1 mobilization required the btgA and btgB genes.

Cloning and expression of BtgA. The predicted amino acid sequence of BtgA revealed a helix-turn-helix DNA binding motif (amino acids 118 to 137) (12). Thisprotein, therefore, seemed a likely candidate for binding to theoriT region. To test this possibility, btgA was cloned into thepET-19b expression vector to give pDHBA and overexpressed in E.coli BL21(DE3). The positions of primers arba5N and arba3B usedto amplify btgA by PCR are illustrated in Fig. 1. DNA sequencingof the entire 630-bp insert and part of the pET-19b promoter sequenceconfirmed that the cloned gene contained no sequence errors. FollowingIPTG induction of pDHBA, an approximately 27-kDa band was visualized(Fig. 2). The predicted mass of BtgA, as determined from the DNAsequence, was 23.2 kDa, or 26.1 kDa with the leader sequence fromthe pET-19b expression vector included. To confirm that this bandrepresented expressed BtgA, the first 24 amino acids of the aminoterminus of the 26.1-kDa protein band were sequenced, revealingthe correct predicted fusion protein.

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FIG. 2. Overproduction and purification of BtgA. Lane 1, Promega mid-range protein molecular mass marker (masses in kilodaltons are shown at the left); lane 2, proteins that did not bind to the His-Tag binding resin following the addition of crude extract; lane 3, BtgA protein eluted from the His-Tag column following multistep dialysis (see Materials and Methods).

BtgA was expressed in E. coli at relatively high levels. Scanning densitometry using an AMBIOS video imaging system to quantitateprotein concentrations in Coomassie brilliant blue-stained SDS-polyacrylamidegels indicated that 10.6% of the total amount of E. coli proteinexpressed was BtgA (data not shown).

Gel mobility shift assay. The BtgA-oriT complex was analyzed in an electrophoretic mobility shift assay to demonstrate noncovalent interaction of BtgAwith the oriT (1, 8). Purified BtgA protein ranging from10 to 300 ng and labeled 304-bp pBFTM10 oriT fragment were incubatedwith a binding buffer and electrophoresed in 5% polyacrylamidegels at 4°C (Fig. 3; see Materials and Methods). Increasing concentrationsof BtgA (10, 50, and 100 ng [Fig. 3, lanes 2 to 4, respectively])demonstrated a concentration-dependent manner of binding withoriT. At 300 ng (lane 5), BtgA demonstrated the maximum shiftof oriT DNA (position A). The presence of poly(dI-dC) at 1 and3 µg failed to disrupt the interaction between the oriT regionand BtgA (lanes 6 and 7, respectively). To demonstrate the specificityof binding, specific competitor pJA-7ZT (containing pBFTM10 oriT)plasmid DNA was added in a 50-fold excess, resulting in partialinhibition of BtgA binding, while 100- and 300-fold excess competitorcompletely inhibited the binding reaction (lanes 8 to 10). Ofnote, storage of BtgA at $-$ 80°C resulted in some loss of bindingactivity after a few days, likely the result of precipitation.

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FIG. 3. Binding of purified BtgA protein to the pBFTM10 oriT. Ten nanograms of 304-bp BamHI pBFTM10 oriT fragment labeled at the 5' terminus with [ $gamma$ -³²P]ATP was incubated with purified BtgA (see Materials and Methods). Lane 1, labeled oriT fragment without addition of protein; lanes 2 to 5, labeled oriT fragment with addition of 10, 50, 100, and 300 ng of purified BtgA protein; lanes 6 and 7, oriT fragment incubated with 300 ng of BtgA in the presence of 1 and 3 µg of poly(dI-dC), respectively; lanes 8 to 10, labeled oriT fragment incubated with 300 ng of BtgA protein plus 50-, 100-, and 300-fold excess cold competitor oriT-containing plasmid pGEM-7ZT, respectively.

DNase I footprinting. DNase I protection experiments were used to localize the precise binding sites of BtgA on the pBFTM10 oriT. The oriT fragmentwas specifically labeled on the upper or lower strand with [ $gamma$ -³²P]ATP and then incubated in the presence of increasing amountsof purified BtgA. These DNA-protein complexes were subjected topartial DNase I digestion to define the binding site(s) of BtgA.The resulting products were separated on 8% polyacrylamide sequencinggels and visualized by autoradiography (Fig. 4). Three distinctregions of protection were visualized on the lower strand. Tworegions, consisting of 36 nucleotides (462 to 498 [Fig. 4A]) and35 nucleotides (501 to 535 [Fig. 4A]), demonstrated the strongestprotection after the addition of $>=$ 0.5 µg of BtgA, while a thirdregion, containing three identifiable nucleotides (536 to 558[Fig. 4A]), demonstrated weaker protection at higher protein concentrations.In addition, 3 nucleotides, 498 to 500, showed weaker protectionand were located between the strongly protected regions. The firstprotected region overlaps the right half of IRI (which containsa consensus sequence for the nick site) and the left half of IRII(Fig. 4 and 5), while the second protected region overlaps theright half of IRII and the left half of IRIII. The third, weakerregion of protection overlaps 10 nucleotides of the right halfof IRIII. Bands at 458 to 461 and 498 to 500 demonstrated possibleminimal protection. No regions of protection were found in theremaining sequence. We detected no regions of protection on theupper strand that would correspond to the protected zones on thelower strand (Fig. 4B).

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FIG. 4. DNase I footprint analysis of the BtgA-pBFTM10 oriT protein complex. The specifically labeled upper and lower strands of oriT were incubated with increasing amounts of purified BtgA protein in binding reactions. The BtgA-oriT complexes were subjected to limited cleavage by DNase I and electrophoresed on 8% polyacrylamide sequencing gels. (A) Cleavage pattern of the lower strand of oriT. Quantities of purified BtgA in reaction mixtures: lane C, none; lanes 1 to 5, 100 ng, 300 ng, 500 ng, 1 µg, and 3 µg, respectively. Locations of the inverted repeats are shown by arrows. L and R designate the left and right arms, respectively, of the repeats. For IRI, only the right arm of the repeat is shown since the region corresponding to the left arm is undetectable under the conditions of the footprint. The locations of DNase I protection regions are indicated at the right by brackets. Asterisks represent the region of weak protection (see Results and Discussion). Nucleotide numbering at the left is from the labeled end and corresponds to the published sequence (12). The inset shows the DNase I digestion pattern up to the top of the gel, indicating that no regions of protection were seen, and also demonstrates that the extents of DNase I digestion were similar for all reactions. (B) Cleavage pattern of the upper strand of oriT. Quantities of BtgA in reaction mixtures: lanes 1 to 6, 100 ng, 300 ng, 500 ng, 1 µg, 2 µg, and 3 µg, respectively; lane C, none.

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FIG. 5. Double-stranded nucleotide sequence of the oriT region of pBFTM10. The dark gray boxed regions on the lower strand indicate regions of BtgA binding, as determined by DNase I protection assays. The light gray box indicates the region of weak binding. The location of a putative nic site based on the consensus sequence (12, 39) is shown, as are the left (L) and right (R) arms of the three inverted repeats and the start codon for btgA.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The conjugative mechanisms required for transfer of plasmids in Bacteroides spp. are not well understood but are presumedto include initiation processes, similar to those of RP4 or theF plasmid (6, 9, 27, 44). Thus, it is presumed thatrelaxosomes are formed prior to transfer of a single strand ofDNA. For RP4, this requires an oriT region, two DNA binding proteins,a stabilizing protein, and a nickase (16, 43). pBFTM10 hasonly two transfer genes, both of which are necessary for DNA transfer.

To further our understanding of the processes required for mobilization of plasmid DNA in Bacteroides spp., we first determinedthe location of the oriT region by testing for mobilization inE. coli. A 304-bp fragment that contained the three sets of invertedrepeats identified previously as likely targets for protein bindingwas chosen. The putative promoter of btgA is immediately downstreamof IRIII and was also included in the cloned fragment. Mobilizationof the oriT region in E. coli was demonstrated only when bothbtgA and btgB were provided in trans, although R751 must alsobe coresident. It is presumed that the role of R751 is to providea transfer apparatus for mobilization of Bacteroides transferfactors, including pGAT400, pB8-51, pLV22a, and the conjugal transposonTn4399, in E. coli (12, 13, 21, 25, 32). However, itwas previously unknown if cotransfer of R751 with these transferfactors was required. Normally R751 transfers at levels $>=$ 1.4 ordersof magnitude greater than those for the coresident transfer factorand has thus been found in transconjugants that received the mobilizedtransfer factor. Indeed, in these studies, R751 was efficientlyself-transferred at levels 1.4 orders of magnitude greater thanthose for the mobilized pGAT400 or pJAYC1 (12, 30). As expected,we observed that 100% of pGAT400 transconjugants also containedR751. However, only 85% of pJAYC1 transconjugants also containedR751. Thus, it appears that cotransfer of R751 is not necessaryfor pJAYC1 mobilization, although it is not known why a differencebetween R751 cotransfer with pGAT400 and pJAYC1 was seen. Thisfinding implies that R751 indeed may simply provide a transferapparatus utilized by pBFTM10 and other transfer factors.

The function of one of the mobilization proteins, BtgA, was tested after cloning, expression, and purification in differentassays with the pBFTM10 oriT. The presence of a helix-turn-helixmotif suggested that BtgA may be a DNA binding protein, and wetested whether it could bind to the pBFTM10 oriT. Electrophoreticmobility shift assays demonstrated significant specific bindingof BtgA to the 304-bp oriT-containing fragment. Poly(dI-dC) inconcentrations of up to 3 µg did not affect the mobility shiftresults. The addition of unlabeled oriT fragment contained inplasmid pJAYC1 was an effective competition for this binding reaction,confirming its specificity (Fig. 3). However, intermediate mobilityshifts were seen at protein concentrations ranging from 10 to100 ng (Fig. 3). These findings could represent the oligomerizationof BtgA either before or during binding. Alternatively, this couldrepresent a concentration-dependent increase in binding to additionalregions within the oriT fragment, as seen for TraK from RP4 (46),and may be supported by the results of DNase I footprinting experiments(see below). Assays to determine if oligomers are involved inbinding should resolve this observation.

DNase I protection assays localized BtgA binding to three regions on the lower strand of the pBFTM10 oriT (Fig. 5). The mostprominent zones of protection were visualized at nucleotides 462to 497 and 501 to 535. Taken together, these two regions span71 nucleotides that cover parts (or all) of the three invertedrepeats within the oriT region. The first region of protectiontoward the 5' terminus of the oriT region includes the right halfof IRI, which also contains the consensus nick site sequence -TTCCTCTTG/C-(39). Results of preliminary experiments using labeled double-strandedlinear oriT DNA combined with BtgA support this observation (unpublisheddata). A weaker zone of protection was visualized on nucleotides536 to 558, which was visualized only with higher concentrationsof protein. No large regions of protection were visualized onthe upper strand of the pBFTM10 oriT, although individual basescould be protected in more compressed areas but not seen. Thisapparent asymmetric binding of BtgA protein to oriT could be dueto a conformational change in the DNA as a result of wrappingor bending during BtgA-oriT interaction. This is not unusual,having been previously observed for single-stranded DNA bindingproteins involved in replication (protection over 70 nucleotideson one strand only [5]) and the E. coli Fpg zinc finger protein(tested by using high-resolution hydroxyl radical footprintinganalysis [35]), as well as several other bacterial and eukaryoticDNA binding proteins (7, 14, 18, 36, 41, 42, 47).

The location of BtgA binding strongly supports its role in DNA processing functions necessary for transfer initiation. Bindingto recognition sequences within the oriT region is necessary forefficient transfer in RP4 and other plasmids. For RP4, TraJ bindsto the right arm of a 19-nucleotide inverted repeat recognizinga 10-bp sequence within 8 nucleotides of the downstream nick site(45). TraJ binding to supercoiled DNA is required for bindingand nicking activity of the relaxase TraI, presumably by conformationalchange of the nick site. TraK is not required for RP4 transferbut increases the efficiency of relaxosome formation. It bindsdownstream of the nick site over an approximate 180-nucleotideregion, which requires as many as 15 to 20 monomers of TraK toform the complex resulting in bending of DNA (46). The preciserole of BtgA in DNA processing has not been defined, but it isrequired for transfer of pBFTM10 (12). The relatively largeregion of protection overlapping the inverted repeats, and possiblenick site, raises the possibility that BtgA is multifunctional.

	ACKNOWLEDGMENTS

This work was supported by Veterans Administration Medical Research Service Merit Review grant 001.

We thank J. Nawrocki, A. Wolfe, S. Baker, C. Hofmann, and V. Bublys for providing various materials or equipment necessaryfor completion of this project. We thank B. Wakim for synthesisand sequencing the amino terminus of BtgA. We thank M. Malamyand C. Murphy for valuable discussions regarding R751 and pDG5mobilization in E. coli.

	FOOTNOTES

^* Corresponding author. Mailing address: Loyola University Chicago, Bldg. 54, Room 101, 2160 S. First Ave., Maywood, IL 60153.Phone: (708) 216-2792. Fax: (708) 216-2269. E-mail: dhecht{at}luc.edu.

Present address: Division of Neonatology, Department of Pediatrics, University of Illinois at Chicago, Chicago, IL 60616.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1998. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.

2. Brook, I. 1989. In vitro susceptibility and in vivo efficacy of antimicrobials in the treatment of Bacteroides fragilis-Escherichia coli infection in mice. J. Infect. Dis. 160:651-656[Medline].

3. Dagert, M., and S. D. Erlich. 1979. Prolonged incubation in calcium chloride improves the competence of Escherichia coli cells. Gene 6:23-28[Medline].

4. Davies, J. 1994. Inactivation of antibiotics and the dissemination of resistance genes. Science 264:375-381[Abstract/Free Full Text].

5. Dimitrova, D. S., M. Giacca, F. Demarchi, G. Biamonti, S. Riva, and A. Falaschi. 1996. In vivo protein-DNA interactions at a human DNA replication origin. Proc. Natl. Acad. Sci. USA 93:1498-1503[Abstract/Free Full Text].

6. Frost, L. S., K. A. Ippen-Ihler, and R. Skurray. 1994. Analysis of the sequence and gene products of the transfer region of the F sex factor. Microbiology 58:162-210.

7. Fu, G. K., and D. M. Markovitz. 1998. The human LON protease binds to mitochondrial promoters in a single-stranded, site specific, strand-specific manner. Biochemistry 37:1905-1909[Medline].

8. Galas, D. J., and A. Schmitz. 1978. Footprinting: a simple method for the detection of protein-DNA binding specificity. Nucleic Acids Res. 5:3157-3170[Abstract/Free Full Text].

9. Gao, Q., Y. Luo, and R. C. Deonier. 1994. Initiation and termination of DNA transfer at F plasmid oriT. Mol. Microbiol. 11:449-458[Medline].

10. Hacker, J., G. Blum-Oehler, I. Muhldorfer, and H. Tschape. 1997. Pathogenicity islands of virulent bacteria: structure, function and impact on microbial evolution. Mol. Microbiol. 23:1089-1097[Medline].

11. Haggoud, A., G. Reyssett, H. Azeddoug, and M. Sebald. 1994. Nucleotide sequence analysis of two 5-nitroimidazole resistance determinants from Bacteroides strains and of a new insertion sequence upstream of the two genes. Antimicrob. Agents Chemother. 38:1047-1051[Abstract/Free Full Text].

12. Hecht, D. W., T. J. Jagielo, and M. H. Malamy. 1991. Conjugal transfer of antibiotic resistance factors in Bacteroides fragilis: the btgA and btgB genes of plasmid pBFTM10 are required for its transfer from Bacteroides fragilis and for its mobilization by IncP $beta$ plasmid R751 in Escherichia coli. J. Bacteriol. 173:7471-7480[Abstract/Free Full Text].

13. Hecht, D. W., and M. H. Malamy. 1989. Tn4399, a conjugal transposable mobilizing element of Bacteroides fragilis. J. Bacteriol. 171:3603-3608[Abstract/Free Full Text].

14. Kaul, R., M. Allen, E. M. Bradbury, and W. M. Wenman. 1996. Sequence specific binding of chlamydial histone H1-like protein. Nucleic Acids Res. 24:2981-2989[Abstract/Free Full Text].

15. Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].

16. Lanka, E., and B. Wilkens. 1995. DNA processing in bacterial conjugation. Annu. Rev. Biochem. 64:141-169[Medline].

17. Lessl, M., and E. Lanka. 1994. Common mechanism in bacterial conjugation and Ti-Mediated T-DNA transfer to plant cells. J. Biol. Chem. 77:321-324.

18. Marr, M. T., and J. W. Roberts. 1997. Promoter recognition as measured by binding of polymerase to non-template strand oligonucleotide. Science 276:1258-1260[Abstract/Free Full Text].

19. Meyer, R. J., and J. A. Shapiro. 1980. Genetic organization of the broad-host-range IncP-1 plasmid R751. J. Bacteriol. 143:1362-1373[Abstract/Free Full Text].

20. Miller, J. H. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

21. Murphy, C. G., and M. H. Malamy. 1993. Characterization of a "mobilization cassette" in transposon Tn4399 from Bacteroides fragilis. J. Bacteriol. 175:5814-5823[Abstract/Free Full Text].

22. Noble, W. C. 1997. Antibiotic resistance in the staphylococci. Sci. Prog. 80:5-20.

23. Novicki, T. J., and D. W. Hecht. 1995. Characterization and DNA sequence of the mobilization region of pLV22a from Bacteroides fragilis. J. Bacteriol. 177:4466-4473[Abstract/Free Full Text].

24. Pansegrau, W., D. Balzer, K. Volker, R. Lurz, and E. Lanka. 1990. In vitro assembly of relaxosomes at the transfer origin of plasmid RP4. Proc. Natl. Acad. Sci. USA 87:6555-6559[Abstract/Free Full Text].

25. Pansegrau, W., and E. Lanka. 1996. Enzymology of DNA transfer by conjugative mechanisms. Prog. Nucleic Acid Res. Mol. Biol. 54:197-251[Medline].

26. Pansegrau, W., W. Schroder, and E. Lanka. 1993. Relaxase (TraI) of IncP $alpha$ plasmid RP4 catalyzes a site-specific cleaving-joining reaction of single-stranded DNA. Proc. Natl. Acad. Sci. USA 90:2925-2929[Abstract/Free Full Text].

27. Pansegrau, W., G. Ziegelin, and E. Lanka. 1990. Covalent association of the TraI gene product of plasmid RP4 with the 5' terminal nucleotide at the relaxation nick site. J. Biol. Chem. 265:10637-10644[Abstract/Free Full Text].

28. Salyers, A. A. 1984. Bacteroides of the human lower intestinal tract. Annu. Rev. Microbiol. 38:293-313[Medline].

29. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

30. Shoemaker, N. B., C. Getty, E. P. Guthrie, and A. A. Salyers. 1986. Regions in Bacteroides plasmids pBFTM10 and pB8-51 that allow Escherichia coli-Bacteroides shuttle vectors to be mobilized by IncP plasmids and by a conjugative Bacteroides tetracycline resistance element. J. Bacteriol. 166:959-965[Abstract/Free Full Text].

31. Smith, C. J. 1985. Characterization of Bacteroides ovatus plasmid pBI136 and structure of its clindamycin resistance region. J. Bacteriol. 161:1069-1073[Abstract/Free Full Text].

32. Smith, C. J., and F. L. Macrina. 1984. Large transmissible clindamycin resistance plasmid in Bacteroides ovatus. J. Bacteriol. 158:739-741[Abstract/Free Full Text].

33. Tally, F. P., and M. H. Malamy. 1982. Mechanism of antimicrobial resistance and resistance transfer in anaerobic bacteria. Scand. J. Infect. Dis. 35:37-44.

34. Tally, F. P., D. R. Snydman, S. L. Gorbach, and M. H. Malamy. 1979. Plasmid-mediated, transferable resistance to clindamycin and erythromycin in Bacteroides fragilis. J. Infect. Dis. 139:83-88[Medline].

35. Tchou, J., M. L. Michaels, J. H. Miller, and A. P. Grollman. 1993. Function of the zinc finger in Escherichia coli Fpg protein. J. Biol. Chem. 268:26738-26744[Abstract/Free Full Text].

36. Tintut, Y., J. T. Wang, and J. D. Gralla. 1995. A novel bacterial transcriptional cycle involving sigma 54. Genes Dev. 9:2305-2313[Abstract/Free Full Text].

37. Trinh, S., A. Haggoud, and G. Reysset. 1996. Conjugal transfer of the 5-nitroimidazole resistance plasmid pIP417 from Bacteroides vulgatus BV-17: characterization and nucleotide sequence analysis of the mobilization region. J. Bacteriol. 178:6671-6676[Abstract/Free Full Text].

38. Trinh, S., and G. Reysset. 1997. Identification and DNA sequence of the mobilization region of the 5-nitroimidazole resistance plasmid pIP421 from Bacteroides fragilis. J. Bacteriol. 179:4071-4074[Abstract/Free Full Text].

39. Waters, V. L., K. H. Hirata, W. Pansegrau, E. Lanka, and D. G. Guiney. 1991. Sequence identity in the nick regions of IncP plasmid transfer origins and T-DNA borders of Agrobacterium Ti plasmids. Proc. Natl. Acad. Sci. USA 88:1456-1460[Abstract/Free Full Text].

40. Welch, R. A., K. R. Jones, and F. L. Macrina. 1979. Transferable lincosamide-macrolide resistance in Bacteroides. Plasmid 2:261-268[Medline].

41. Wells, J., P. Held, S. Illenye, and N. H. Heintz. 1996. Protein-DNA interactions at the major and minor promoters of the divergently transcribed dhfr and rep3 genes during the Chinese hamster ovary cell cycle. Mol. Cell. Biol. 16:634-647[Abstract].

42. Werel, W., P. Schickor, and H. Heumann. 1991. Flexibility of the DNA enhances promoter affinity of Escherichia coli RNA polymerase. EMBO J. 10:2589-2594[Medline].

43. Wilkens, B., and E. Lanka. 1993. DNA processing and replication during plasmid transfer between Gram-negative bacteria. In D. B. Clewell (ed.), Bacterial conjugation. Plenum Press, New York, N.Y.

44. Willets, N., and R. Skurray. 1987. Structure and function of the F factor and mechanisms of conjugation, p. 1110-1113. In F. C. Neidhardt, J. L. Ingraham, K. B. Low, B. Magasanik, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella typhimurium: cellular and molecular biology. American Society for Microbiology, Washington, D.C.

45. Ziegelin, G., J. P. Furste, and E. Lanka. 1989. TraJ protein of plasmid Rp4 binds to a 19 base pair invert sequence repetition within the transfer origin. J. Biol. Chem. 264:11989-11994[Abstract/Free Full Text].

46. Ziegelin, G., W. Pansegrau, R. Lurz, and E. Lanka. 1992. TraK protein of conjugative plasmid RP4 forms a specialized nucleoprotein complex with the transfer origin. J. Biol. Chem. 267:17279-17286[Abstract/Free Full Text].

47. Zou, Y., R. Walker, H. Bassett, N. E. Geacintov, and B. VanHouten. 1997. Formation of DNA repair intermediates and excision by the ATP-dependent Uvr-UvrC endonuclease. J. Biol. Chem. 272:4820-4827[Abstract/Free Full Text].

This article has been cited by other articles:

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Vedantam, G., Hecht, D. W. (2002). Isolation and Characterization of BTF-37: Chromosomal DNA Captured from Bacteroides fragilis That Confers Self-Transferability and Expresses a Pilus-Like Structure in Bacteroides spp. and Escherichia coli. J. Bacteriol. 184: 728-738 [Abstract] [Full Text]

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1.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1998. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.
2.	Brook, I. 1989. In vitro susceptibility and in vivo efficacy of antimicrobials in the treatment of Bacteroides fragilis-Escherichia coli infection in mice. J. Infect. Dis. 160:651-656[Medline].
3.	Dagert, M., and S. D. Erlich. 1979. Prolonged incubation in calcium chloride improves the competence of Escherichia coli cells. Gene 6:23-28[Medline].
4.	Davies, J. 1994. Inactivation of antibiotics and the dissemination of resistance genes. Science 264:375-381[Abstract/Free Full Text].
5.	Dimitrova, D. S., M. Giacca, F. Demarchi, G. Biamonti, S. Riva, and A. Falaschi. 1996. In vivo protein-DNA interactions at a human DNA replication origin. Proc. Natl. Acad. Sci. USA 93:1498-1503[Abstract/Free Full Text].
6.	Frost, L. S., K. A. Ippen-Ihler, and R. Skurray. 1994. Analysis of the sequence and gene products of the transfer region of the F sex factor. Microbiology 58:162-210.
7.	Fu, G. K., and D. M. Markovitz. 1998. The human LON protease binds to mitochondrial promoters in a single-stranded, site specific, strand-specific manner. Biochemistry 37:1905-1909[Medline].
8.	Galas, D. J., and A. Schmitz. 1978. Footprinting: a simple method for the detection of protein-DNA binding specificity. Nucleic Acids Res. 5:3157-3170[Abstract/Free Full Text].
9.	Gao, Q., Y. Luo, and R. C. Deonier. 1994. Initiation and termination of DNA transfer at F plasmid oriT. Mol. Microbiol. 11:449-458[Medline].
10.	Hacker, J., G. Blum-Oehler, I. Muhldorfer, and H. Tschape. 1997. Pathogenicity islands of virulent bacteria: structure, function and impact on microbial evolution. Mol. Microbiol. 23:1089-1097[Medline].
11.	Haggoud, A., G. Reyssett, H. Azeddoug, and M. Sebald. 1994. Nucleotide sequence analysis of two 5-nitroimidazole resistance determinants from Bacteroides strains and of a new insertion sequence upstream of the two genes. Antimicrob. Agents Chemother. 38:1047-1051[Abstract/Free Full Text].
12.	Hecht, D. W., T. J. Jagielo, and M. H. Malamy. 1991. Conjugal transfer of antibiotic resistance factors in Bacteroides fragilis: the btgA and btgB genes of plasmid pBFTM10 are required for its transfer from Bacteroides fragilis and for its mobilization by IncP $beta$ plasmid R751 in Escherichia coli. J. Bacteriol. 173:7471-7480[Abstract/Free Full Text].
13.	Hecht, D. W., and M. H. Malamy. 1989. Tn4399, a conjugal transposable mobilizing element of Bacteroides fragilis. J. Bacteriol. 171:3603-3608[Abstract/Free Full Text].
14.	Kaul, R., M. Allen, E. M. Bradbury, and W. M. Wenman. 1996. Sequence specific binding of chlamydial histone H1-like protein. Nucleic Acids Res. 24:2981-2989[Abstract/Free Full Text].
15.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].
16.	Lanka, E., and B. Wilkens. 1995. DNA processing in bacterial conjugation. Annu. Rev. Biochem. 64:141-169[Medline].
17.	Lessl, M., and E. Lanka. 1994. Common mechanism in bacterial conjugation and Ti-Mediated T-DNA transfer to plant cells. J. Biol. Chem. 77:321-324.
18.	Marr, M. T., and J. W. Roberts. 1997. Promoter recognition as measured by binding of polymerase to non-template strand oligonucleotide. Science 276:1258-1260[Abstract/Free Full Text].
19.	Meyer, R. J., and J. A. Shapiro. 1980. Genetic organization of the broad-host-range IncP-1 plasmid R751. J. Bacteriol. 143:1362-1373[Abstract/Free Full Text].
20.	Miller, J. H. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
21.	Murphy, C. G., and M. H. Malamy. 1993. Characterization of a "mobilization cassette" in transposon Tn4399 from Bacteroides fragilis. J. Bacteriol. 175:5814-5823[Abstract/Free Full Text].
22.	Noble, W. C. 1997. Antibiotic resistance in the staphylococci. Sci. Prog. 80:5-20.
23.	Novicki, T. J., and D. W. Hecht. 1995. Characterization and DNA sequence of the mobilization region of pLV22a from Bacteroides fragilis. J. Bacteriol. 177:4466-4473[Abstract/Free Full Text].
24.	Pansegrau, W., D. Balzer, K. Volker, R. Lurz, and E. Lanka. 1990. In vitro assembly of relaxosomes at the transfer origin of plasmid RP4. Proc. Natl. Acad. Sci. USA 87:6555-6559[Abstract/Free Full Text].
25.	Pansegrau, W., and E. Lanka. 1996. Enzymology of DNA transfer by conjugative mechanisms. Prog. Nucleic Acid Res. Mol. Biol. 54:197-251[Medline].
26.	Pansegrau, W., W. Schroder, and E. Lanka. 1993. Relaxase (TraI) of IncP $alpha$ plasmid RP4 catalyzes a site-specific cleaving-joining reaction of single-stranded DNA. Proc. Natl. Acad. Sci. USA 90:2925-2929[Abstract/Free Full Text].
27.	Pansegrau, W., G. Ziegelin, and E. Lanka. 1990. Covalent association of the TraI gene product of plasmid RP4 with the 5' terminal nucleotide at the relaxation nick site. J. Biol. Chem. 265:10637-10644[Abstract/Free Full Text].
28.	Salyers, A. A. 1984. Bacteroides of the human lower intestinal tract. Annu. Rev. Microbiol. 38:293-313[Medline].
29.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
30.	Shoemaker, N. B., C. Getty, E. P. Guthrie, and A. A. Salyers. 1986. Regions in Bacteroides plasmids pBFTM10 and pB8-51 that allow Escherichia coli-Bacteroides shuttle vectors to be mobilized by IncP plasmids and by a conjugative Bacteroides tetracycline resistance element. J. Bacteriol. 166:959-965[Abstract/Free Full Text].
31.	Smith, C. J. 1985. Characterization of Bacteroides ovatus plasmid pBI136 and structure of its clindamycin resistance region. J. Bacteriol. 161:1069-1073[Abstract/Free Full Text].
32.	Smith, C. J., and F. L. Macrina. 1984. Large transmissible clindamycin resistance plasmid in Bacteroides ovatus. J. Bacteriol. 158:739-741[Abstract/Free Full Text].
33.	Tally, F. P., and M. H. Malamy. 1982. Mechanism of antimicrobial resistance and resistance transfer in anaerobic bacteria. Scand. J. Infect. Dis. 35:37-44.
34.	Tally, F. P., D. R. Snydman, S. L. Gorbach, and M. H. Malamy. 1979. Plasmid-mediated, transferable resistance to clindamycin and erythromycin in Bacteroides fragilis. J. Infect. Dis. 139:83-88[Medline].
35.	Tchou, J., M. L. Michaels, J. H. Miller, and A. P. Grollman. 1993. Function of the zinc finger in Escherichia coli Fpg protein. J. Biol. Chem. 268:26738-26744[Abstract/Free Full Text].
36.	Tintut, Y., J. T. Wang, and J. D. Gralla. 1995. A novel bacterial transcriptional cycle involving sigma 54. Genes Dev. 9:2305-2313[Abstract/Free Full Text].
37.	Trinh, S., A. Haggoud, and G. Reysset. 1996. Conjugal transfer of the 5-nitroimidazole resistance plasmid pIP417 from Bacteroides vulgatus BV-17: characterization and nucleotide sequence analysis of the mobilization region. J. Bacteriol. 178:6671-6676[Abstract/Free Full Text].
38.	Trinh, S., and G. Reysset. 1997. Identification and DNA sequence of the mobilization region of the 5-nitroimidazole resistance plasmid pIP421 from Bacteroides fragilis. J. Bacteriol. 179:4071-4074[Abstract/Free Full Text].
39.	Waters, V. L., K. H. Hirata, W. Pansegrau, E. Lanka, and D. G. Guiney. 1991. Sequence identity in the nick regions of IncP plasmid transfer origins and T-DNA borders of Agrobacterium Ti plasmids. Proc. Natl. Acad. Sci. USA 88:1456-1460[Abstract/Free Full Text].
40.	Welch, R. A., K. R. Jones, and F. L. Macrina. 1979. Transferable lincosamide-macrolide resistance in Bacteroides. Plasmid 2:261-268[Medline].
41.	Wells, J., P. Held, S. Illenye, and N. H. Heintz. 1996. Protein-DNA interactions at the major and minor promoters of the divergently transcribed dhfr and rep3 genes during the Chinese hamster ovary cell cycle. Mol. Cell. Biol. 16:634-647[Abstract].
42.	Werel, W., P. Schickor, and H. Heumann. 1991. Flexibility of the DNA enhances promoter affinity of Escherichia coli RNA polymerase. EMBO J. 10:2589-2594[Medline].
43.	Wilkens, B., and E. Lanka. 1993. DNA processing and replication during plasmid transfer between Gram-negative bacteria. In D. B. Clewell (ed.), Bacterial conjugation. Plenum Press, New York, N.Y.
44.	Willets, N., and R. Skurray. 1987. Structure and function of the F factor and mechanisms of conjugation, p. 1110-1113. In F. C. Neidhardt, J. L. Ingraham, K. B. Low, B. Magasanik, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella typhimurium: cellular and molecular biology. American Society for Microbiology, Washington, D.C.
45.	Ziegelin, G., J. P. Furste, and E. Lanka. 1989. TraJ protein of plasmid Rp4 binds to a 19 base pair invert sequence repetition within the transfer origin. J. Biol. Chem. 264:11989-11994[Abstract/Free Full Text].
46.	Ziegelin, G., W. Pansegrau, R. Lurz, and E. Lanka. 1992. TraK protein of conjugative plasmid RP4 forms a specialized nucleoprotein complex with the transfer origin. J. Biol. Chem. 267:17279-17286[Abstract/Free Full Text].
47.	Zou, Y., R. Walker, H. Bassett, N. E. Geacintov, and B. VanHouten. 1997. Formation of DNA repair intermediates and excision by the ATP-dependent Uvr-UvrC endonuclease. J. Biol. Chem. 272:4820-4827[Abstract/Free Full Text].