Fur Is a Repressor of Biofilm Formation in Yersinia pestis

Background Yersinia pestis synthesizes the attached biofilms in the flea proventriculus, which is important for the transmission of this pathogen by fleas. The hmsHFRS operons is responsible for the synthesis of exopolysaccharide (the major component of biofilm matrix), which is activated by the signaling molecule 3′, 5′-cyclic diguanylic acid (c-di-GMP) synthesized by the only two diguanylate cyclases HmsT, and YPO0449 (located in a putative operonYPO0450-0448). Methodology/Principal Findings The phenotypic assays indicated that the transcriptional regulator Fur inhibited the Y. pestis biofilm production in vitro and on nematode. Two distinct Fur box-like sequences were predicted within the promoter-proximal region of hmsT, suggesting that hmsT might be a direct Fur target. The subsequent primer extension, LacZ fusion, electrophoretic mobility shift, and DNase I footprinting assays disclosed that Fur specifically bound to the hmsT promoter-proximal region for repressing the hmsT transcription. In contrast, Fur had no regulatory effect on hmsHFRS and YPO0450-0448 at the transcriptional level. The detection of intracellular c-di-GMP levels revealed that Fur inhibited the c-di-GMP production. Conclusions/Significance Y. pestis Fur inhibits the c-di-GMP production through directly repressing the transcription of hmsT, and thus it acts as a repressor of biofilm formation. Since the relevant genetic contents for fur, hmsT, hmsHFRS, and YPO0450-0448 are extremely conserved between Y. pestis and typical Y. pseudotuberculosis, the above regulatory mechanisms can be applied to Y. pseudotuberculosis.


Introduction
Y. pestis is highly virulent to mammalians including humans, and causes systemic and fatal infections mainly manifested as bubonic, septicemic, and pneumonic plague. Y. pestis is primarily transmitted via the bite of an infected flea. Y. pestis synthesizes the attached biofilms in the flea proventriculus, making the blockage of fleas [1,2]. The blockage of fleas makes them feel hungry and repeatedly attempt to feed, and thus, the plague bacilli will be pumped into the host body during the futile feeding attempts, promoting the bacterial transmission between mammalian reservoirs [1,2].
The Yersinia biofilms are a population of bacterial colonies embedded in the self-synthesized extracellular matrix, and the matrix is primarily composed of exopolysaccharide that is the homopolymer of N-acetyl-D-glucosamine [1]. The hmsHFRS operon is responsible for the synthesis and translocation of biofilm exopolysaccharide across the cell envelope, and all the four genes in this operon are required for the biofilm formation and for the flea blockage [1,3].
The signaling molecule 39, 59-cyclic diguanylic acid (c-di-GMP) is a central positive activator of the enzymes catalyzing the production of biofilm exopolysaccharide [4]. HmsT [5,6] and YPO0449 (y3730 in KIM) [7,8] are the only two diguanylate cyclase enzymes in Y. pestis to synthesize c-di-GMP, and both of them stimulate the Yersinia biofilm formation. The predominant effect of HmsT was on the in vitro biofilm formation, while the role of YPO0449 in the biofilm production is much greater in the flea than in vitro [7]. The Rcs phosphorelay system negatively controls Yersinia biofilm production in both nematode and flea models [9]. The Rcs system is composed of the sensor kinase RcsC, the phosphotransfer RcsD, and the cytoplasmic response regulator RcsB [10]. RcsC and RcsD transfers phosphate to RcsB, and the phosphorylated RcsB (RcsB-P) binds to some of its target promoters to mediate the gene regulation, whereas a complex of RcsB-P and its accessory protein RcsA is required for the regulation of other target genes [10]. The RcsAB box sequence TAAGAAT-ATTCTTA is a 14 bp inverted repeat [11].
The ferric uptake regulator (Fur) is a predominant ironregulating system in bacteria [12]. Fur directly controls not only almost of the iron assimilation functions but a variety of genes involved in various non-iron functions, and thus, this regulator governs a complex regulatory cascade in Y. pestis [13,14]. Two consensus constructs, a 19 bp box and a position-specific scoring matrix (PSSM), have been built to represent the conserved cisacting signals recognized by Fur [13]. The Fur box sequence AATGATAATNATTATCATT is a 9-1-9 inverted repeat.
During the general maintenance of Y. pestis on the agar media, we found that the fur mutant exhibited a much more rugose and dry colony morphology relative to its parent strain, which promoted us to hypothesize the Fur-mediated repression of exopolysaccharide synthesis and biofilm production in Y. pestis (see below for details). In the present work, the detection of biofilms verified that Fur inhibited the Y. pestis biofilm production in vitro and on nematode. The subsequent gene regulation experiments disclosed that Fur specifically bound to the promoter-proximal region of hmsT for repressing the hmsT transcription, and yet, it had no regulatory effect on hmsHFRS and YPO0450-0448. In addition, the detection of intracellular levels of c-di-GMP revealed that Fur inhibited the c-di-GMP production. Therefore, Y. pestis Fur inhibited the c-di-GMP production through directly repressing the transcription of hmsT, and thus, it acted as a repressor of biofilm formation.

Bacterial Strains and Growth
The wild-type (WT) Y. pestis biovar Microtus strain 201 is avirulent to humans but highly lethal to mice [15]. The entire coding region of fur or the base pairs 146 to 468 of hmsS was replaced by the kanamycin resistance cassette by using the onestep inactivation method based on the lambda phage recombination system, to generate the fur or hmsS null mutant (designated as Dfur or DhmsS, respectively) of Y. pestis, as described previously [14]. All the primers used in this study were listed in Table 1. Given the pervious observation that the deletion of hmsS lead to a biofilm-defective phenotype in Y. pestis [16], DhmsS was used as a reference biofilm-defective strain in this work.
A PCR-generated DNA fragment containing the fur coding region together with its promoter-proximal region (458 bp upstream the coding sequence) and transcriptional terminator (189 bp downstream) was cloned into the pACYC184 vector (GenBank accession number X06403) that harbors a chloramphenicol resistance gene. Upon being verified by DNA sequencing, the recombinant plasmid was introduced into Dfur, yielding the complemented mutant strain C-fur.
The incubation temperature of 26uC was employed for the Y. pestis cultivation, unless otherwise specifically indicated. For the general bacterial cultivation and maintenance, Y. pestis was cultivated in the Luria-Bertani (LB) broth or on the LB agar plate. For preparing the glycerol stocks of bacterial cells, a single colony was inoculated on the LB agar plate for further incubation for 1 to 2 d; the bacterial cells were washed into the LB broth at an optical density at 620 nm (OD 620 ) of about 1.5, and stored with addition of 30% glycerol at 280uC. For primer extension or LacZ fusion, 200 ml of bacterial glycerol stocks were inoculated into 18 ml of fresh LB broth, and allowed to grow with shaking at 230 rpm to an OD 620 of 0.4 to 0.5 prior to the bacterial harvest.

RNA Isolation and Primer Extension Assay
Before bacterial harvest, double-volume RNAprotect Bacteria Reagent (Qiagen) was added immediately to each cell culture.
Total bacterial RNAs were extracted using the TRIzol Reagent (Invitrogen) [17]. RNA quality was monitored by agarose gel electrophoresis, and RNA quantity was determined by spectrophotometry. For the primer extension assay [17], an oligonucleotide primer complementary to a portion of the RNA transcript of each indicated gene was employed to synthesize cDNAs from the RNA templates. One to 10 mg of total RNA from each strain was annealed with 1 pmol of [c-32 P] end-labeled reverse primer using a Primer Extension System (Promega) according to the manufacturer's instructions. The same labeled primer was also used for sequencing with the fmolH DNA Cycle Sequencing System (Promega). The primer extension products and sequencing materials were concentrated and analyzed in a 6% polyacrylamide/8 M urea gel. The result was detected by autoradiography (Kodak film).

LacZ Reporter Fusion and b-Galactosidase Assay
The promoter-proximal DNA region of each gene tested was prepared by PCR with the Takara ExTaq DNA polymerase by using Y. pestis 201 genome DNA as template, and then cloned directionally into the HindIII-BamHI site of the transcriptional fusion vector pRW50 [18] that contained a promotorless lacZ reporter gene. Correct clone was verified by DNA sequencing.
Each Y. pestis strain tested was transformed with the recombinant plasmids. The empty plasmid was also introduced into each strain as negative control. The b-Galactosidase activity was measured on cellular extracts from cells cultivated as above by using the b-Galactosidase Enzyme Assay System (Promega) [17].

Preparation of 66His-tagged Fur (His-Fur) Protein
To prepare a His-Fur protein [14], the entire coding region of fur was amplified from Y. pestis 201 and cloned directionally into the BamHI and HindIII site of plasmid pET28a (Novagen), which was verified by DNA sequencing. The recombinant plasmids encoding the His-Fur protein were transformed into Escherichia coli BL21 (DE3) cells (Novagen). Expression of His-Fur protein was induced by addition of 1 mM isopropyl-beta-D-thiogalactoside. The His-Fur protein was purified under native conditions with a QIAexpressionist TM Ni-NTA affinity chromatography (Qiagen). The purified, eluted protein was concentrated with the Amicon Ultra-15 (Millipore) to a final concentration of about 0.1 to 0.3 mg/ml in the storage buffer (PBS, pH 7.5 plus 20% glycerol). The protein purity was verified by SDS-PAGE with silver staining. The purified protein was stored at 280uC.

Electrophoretic Mobility Shift Assay (EMSA)
For EMSA [14], promoter-proximal DNA regions were prepared by PCR amplification for EMSA. EMSA was performed using the Gel Shift Assay Systems (Promega). The 59 ends of DNA were labeled using [c-32 P] ATP and T4 polynucleotide kinase. DNA binding was performed in a 10 ml volume containing binding buffer [100 mM MnCl 2 , 1 mM MgCl 2 , 0.5 mM DTT, 50 mM KCl, 10 mM Tris-HCl (pH 7.5), 0.05 mg/ml sheared salmon sperm DNA, 0.05 mg/ml BSA and 4% glycerol], labeled DNA (1000 to 2000 c.p.m/ml) and increasing amounts of His-Fur. We still included two control reactions: one contained the specific DNA competitor (unlabeled promoter DNA regions; cold probe), while the other was the non-specific protein competitor (rabbit anti-F1-protein polyclonal IgG antibody). After incubation at room temperature for 30 min, the products were loaded onto a native 4% (w/v) polyacrylamide gel and electrophoresed in 0.56TB buffer containing 100 mM MnCl 2 for 30 min at 220 V. Radioactive species were detected by autoradiography.

DNase I Footprinting
For DNase I footprinting [14], promoter-proximal DNA regions were prepared by PCR amplification performed with specific primer pairs including a 59-32 P-labeled forward or reverse one and its non-labeled counterpart. The PCR products were purified using Qiaquick columns (Qiagen). Increasing amount of purified His-protein was incubated with the labeled DNA fragment (2 to 5 pmol) for 30 min at room temperature in a final volume of 10 ml containing binding buffer same as EMSA. Before DNA digestion, 10 ml of Ca 2+ /Mg 2+ solution (5 mM CaCl 2 and 10 mM MgCl 2 ) was added, followed by incubation for 1 min at room temperature. Then, the optimized RQ1 RNase-Free DNase I (Promega) was added to the reaction mixture, and the mixture was incubated at room temperature for 30 to 90 s. The cleavage reaction was stopped by adding 9 ml of the stop solution (200 mM NaCl, 30 mM EDTA and 1% SDS) followed by DNA extraction and precipitation. The partially digested DNA samples were then analyzed in a 6% polyacrylamide/8 M urea gel. Protected regions were identified by comparison with the sequence ladders. For sequencing, the fmolH DNA Cycle Sequencing System (Promega) was used. The result was detected by autoradiography (Kodak film).

Crystal Violet (CV) Staining of Biofilms
Two-hundred microlitre of bacterial glycerol stocks were spotted on the LB agar plate for further incubation for 1 to 2 d. The resulting bacterial cells were washed into the LB broth with an OD 620 value of at least 1.0, stored at 4uC for cold shock for 8 to 12 h, and then diluted to an OD 620 value of 0.8 with fresh LB broth. The diluted cultures were transferred into the 24-well tissue culture plates with 1 ml of cultures in each well, and allowed to grow at 230 rpm for 24 h. The media containing the planktonic cells were removed for determining the OD 620 values. The well with the adherent biofilms was gently washed three times with 2 ml of H 2 O, and then incubated at 80uC for 15 min for the fixation of attached cells. The surface-attached cells were stained with 2 ml of 0.1% crystal violet for 15 min. The solution was removed, and the well was washed three times with 2 ml of H 2 O. Bound dye in the well was dissolved with 3 ml of dimethylsulfoxide. The OD 570 values were recorded to indicate the crystal violet staining. The OD 570 /OD 620 values were calculated to indicate the relative biofilm formation. The OD 620 values were used for normalization to avoid the effect of growth rate and cell density.

Caenorhabditis Elegans Biofilm Assays
The lawns of biofilm-negative Escherichia coli OP50, a uracil auxotroph whose growth was limited on the NGM (Nematode Growth Medium) agar plates, were used as the standard foods for C. elegans. When the larvae or adults of C. elegans grow on the lawns of Y. pestis, this bacterium creates biofilms to cover primarily on the nematode head by blanketing the mouth and thus inhibiting the nematode feeding, which has been developed as a model for Yersinia biofilm research [19,20]. Bacterial strains were transformed with the pBC-GFP vector [21] to generate Y. pestis WT-GFP, Dfur-GFP, DhmsS-GFP, and E. coli OP50-GFP, respectively. To make the bacterial lawns, 200 ml of bacterial glycerol stocks were spotted on the LB agar plate for further incubation for 1 to

Colony Morphology Assay
Aliquots of 5 ml of bacterial glycerol stocks were spotted on the LB plate, followed by the incubation for one week. The photograph of surface morphology of each bacterial colony was recorded.

Determination of Intracellular Levels of c-di-GMP
The intracellular levels of c-di-GMP were determined by a chromatography-coupled tandem mass spectrometry (HPLC-MS/ MS) method as described previously [22]. Two-hundred microlitre of bacterial glycerol stocks were spotted on the LB agar plate for further incubation for 1 to 2 d. The resulting bacterial cells were washed into the LB broth with an OD 620 value of about 0.5, and then aliquots of 5 ml were harvested for the extraction of c-di-GMP with the extraction solvent (acetonitrile: methanol:water = 40:40:20, v/v/v). The chromatographic separation was performed on a Spark HPLC system equipped with a binary pump system and a 200 ml sample loop. The analyte detection was performed on an API 4000-QTRAP quadrupole mass spectrometer equipped with an electro spray ionization source (Applied Biosystems).The serially diluted water solutions of HPLC-grade cdi-GMP (KeraFAST) were used for determining the standard curves. The HPLC-grade xanthosine 39,59-cyclic monophosphate (c-XMP, Sigma) was added as the internal standard into the c-di-GMP extract or standard solution at a final concentration of 50 ng/ml. Aliquots of 1 ml of bacterial cultures were harvest, and the amount of whole-cell protein was determined with a Micro BCA Protein Assay Kit (Thermo Scientific). The final c-di-GMP concentrations were expressed as pmol/mg of bacterial protein.

Experimental Replicates and Statistical Methods
For phenotypic assays and LacZ fusion, experiments were performed with at least three independent bacterial cultures, and the values were expressed as mean 6 standard deviation. Paired Student's t-test was performed to determine statistically significant differences, and P,0.01 was considered to indicate statistical significance. For primer extension, EMSA, and DNase I footprinting, the representative data from at least two independent biological replicates were shown.

Computational Promoter Analysis
The 300 bp upstream regions of the genes tested (Table 2) were retrieved with the 'retrieve-seq' program [23]. The PSSM [13] representing the conserved signals for Fur recognition in Y. pestis was used for the pattern matching within the target upstream DNA regions, by using the matrices-paster tool [23].

Fur Inhibited Biofilm Formation
Growing in the polystyrene microtiter plate, Y. pestis cells tend to attach to the walls [9]. The attached biomass (i.e., in vitro biofilms) can be detected with CV staining, which has been developed long time ago as a model for the determination of in vitro biofilms [24]. Herein, Dfur gave the normalized CV staining significantly greater than WT that was comparable to the complemented mutant C-fur, while the biofilm-negative strain DhmsS gave almost no CV straining (Fig. 1a).
Biofilm-forming bacteria growing on the agar plate can give a rugose colony morphology in which the cells are embedded in abundant biofilm exopolysaccharide, and the degrees of rugose colony morphology positively reflect the ability to synthesize the biofilm exopolysaccharide [9,25,26]. Dfur produced colonies with much more rugose morphology in relative to WT that was comparable to C-fur, while DhmsS made the smooth colonies (Fig. 1b). These suggested that Dfur overproduced the biofilm exopolysaccharide relative to WT.
Yersinia biofilms adhere to the surface of C. elegans, primarily on the head to cover the mouth. When the adult or L4 nematodes were placed on the lawn of Y. pestis expressing GFP and allowed to grow for 12 h, Dfur-GFP produced more extensive and denser biofilms than WT-GFP, while no biofilm was detectable for DhmsS-GFP (negative control) and E. coli OP50 (blank control) (Fig. 1c).
Taken together, Y. pestis Fur acted as a repressor for the biofilm formation, most likely through inhibiting the production of biofilm exopolysaccharide.

hmsT was Predicted to be a Direct Fur Target
The Fur PSSM [13] was used to statistically predict the presence of Fur box-like elements [14] within the promoterproximal regions of the three major biofilm-required loci hmsHFRS, hmsT, and YPO0450-0448. This analysis generated a weight score for each target promoter, and the higher score value indicated the higher probability of the Fur-promoter association [14]. When a frequently used score of 7 was taken as the cutoff value, Fur box-like sequences were found for hmsT rather than the remaining two (Table 2). This computational promoter analysis suggested that Fur could recognize the hmsT promoter for transcriptional regulation.

Fur Repressed hmsT Transcription in a Direct Manner
The primer extension experiments (Fig. 2a) were conducted to determine the yield of primer extension product of hmsT (i.e., the relative hmsT transcription level) in WT or Dfur. A single transcriptional start site was detected to be located at the nucleotide A that was 128 bp upstream of hmsT, and thus, a single promoter was transcribed for hmsT. The primer extension assay also disclosed that the mRNA level of hmsT considerably enhanced in Dfur relative to WT.
To test the action of Fur on the promoter activity of hmsT, we constructed an hmsT::lacZ fusion vector, containing a 453 bp promoter-proximal region of hmsT and the promoterless lacZ, which was then transformed into WT or Dfur (Fig. 2b). The bgalactosidase activity was measured for evaluating the hmsT promoter activity in each strain. The LacZ fusion experiments disclosed that the hmsT promoter activity significantly enhanced in Dfur relative to WT.
EMSA was conducted to answer whether Fur would bind to the hmsT upstream region in vitro (Fig. 2c). As expected, a purified His-Fur bound to the labeled hmsT promoter DNA in a dosedependent manner. To confirm the specificity of Fur-DNA association, the EMSA experiments still included a partial coding region of the 16S rRNA gene, and the negative results were obtained.
In order to locate the precise Fur sites, DNase I footprinting experiments were performed with both coding and non-coding strands of target DNA fragments (Fig. 2d). Since two Fur boxlike sequences were predicted for hmsT, two distinct hmsT promoter-proximal regions, containing the above predicted elements respectively, were subjected to the footprinting experiments. The results confirmed the binding of His-Fur to the two target DNA fragments in vitro. His-Fur protected a Figure 1. Yersinia pestis biofilms assays. a) Adherent bacterial biomass determined by crystal violet staining. Y. pestis was grown in the 24-well polystyrene dishes, and the biomass adherent to the well wall was stained with crystal violet to determine the OD 570 values. The planktonic cells were subjective to determine the OD 620 values (i.e., cell density) for normalization. Shown were the OD 570 /OD 620 values representing the relative capacity of biofilm formation of each strain tested. b) Bacterial colony morphology. Aliquots of 5 ml of bacterial glycerol stocks were spotted on the LB plate, followed by the incubation for one week. c) Yersinia biofilms on C. elegans. The adult or L4 nematodes were spread on the lawn of Y. pestis expressing GFP and allowed to grow for 12 h. Shown were biofilms attach to the head posterior to the nematode mouth. doi:10.1371/journal.pone.0052392.g001 single region within each of the two target DNA fragments tested against DNase I digestion in a dose-dependent pattern. The two footprints were located from 283 to 244 bp (site 2) and from 102 to 71 bp (site 1) upstream of hmsT, respectively. Both of them contained the Fur box-like sequences, and were considered as the Fur sites for hmsT (Fig. 2e).

Fur had no Regulatory Effect on hmsHFRS and YPO0450-0448
The gene regulation experiments still included the first genes (hmsH and YPO0450) of the hmsHFRS and YPO0450-0448 operons. The primer extension (Fig. 3a and 4a) and LacZ fusion ( Fig. 3b and 4b) assays were conducted for hmsH and YPO0450. It was revealed that the fur null mutation have no influence on the hmsH/YPO0450 transcription (Fig. 3a and 4a) or on the hmsH/ YPO0450 promoter activity (Fig. 3b and 4b). In addition, the EMSA experiments ( Fig. 3c and 4c) indicated that His-Fur could not bind to the upsteam DNA regions of hmsH and YPO0450. Therefore, the Fur regulator had no regulatory action on hmsHFRS and YPO0450-0448 at the transcriptional level under the growth conditions tested herein.

Fur Repressed c-di-GMP Production
The intracellular levels of c-di-GMP were determined in WT and Dfur by a HPL-MC/MS method. Compared to WT, a significantly enhanced production of c-di-GMP was observed for Dfur (Fig. 5). These results verified that the Fur-mediated transcriptional repression hmsT accounted for the inhibition of cdi-GMP synthesis by Fur in Y. pestis.

Discussion
Y. pestis is a recently (from the evolutionary point of view) merged clone of the mild enteric pathogen Y. pseudotuberculosis [27]. Y. pseudotuberculosis is transmitted by the food-borne route, while Y. pestis utilizes a radically different mechanism of transmission that rely primarily upon bite of fleas [28]. All of the known structural genes required for the biofilm formation are harbored in Y. pseudotuberculosis, but typical Y. pseudotuberculosis cannot synthesize adhesive biofilms on nematodes and make blockage in fleas [29].
The Y. pseudotuberculosis NghA is a glycosyl hydrolase that cleaves the b-linked N-acetylglucosamine residues, and thus, it plays a key role in degrading the biofilm exopolysaccharide [30]. The RcsAB box-like sequence can be predicted within the promoter-proximal regions of hmsT (Fig. 2e), hmsHFRS (Fig. 3e), and YPO0450-0448 (Fig. 4e). Repression of the hmsT transcription by RcsAB through the RcsAB-promoter association has been established recently [31]. hmsHFRS and YPO0450-044 appears to be the additional direct RcsAB targets (unpublished data), and thus, RcsAB acts as a repressor of Yersinia biofilm formation through inhibiting the production of both c-di-GMP and biofilm exopolysaccharide.
Data presented here disclosed that the Fur regulator had a negative effect on the biofilm formation through repressing the hmsT transcription. DNase I footprinting experiments precisely determined the Fur sites for hmsT. The primer extension assays mapped a single promoter transcribed for hmsT, and accordingly, the core promoter 210 and 235 elements for RNA polymerase recognition were predicted. Collection of data on the translation/ transcription start sites, Shine-Dalgarno (SD) sequence (a ribosomal binding site in the mRNA), core promoter 210 and 235 elements for RNA polymerase recognition, and two cis-acting sites for Fur recognition, enabled us to depict the organization of Furdependent promoter of hmsT herein (Fig. 2e).
The two Fur sites were located downstream and upstream of the transcription start site of hmsT, respectively, while the RcsAB boxlike sequence overlapped the hmsT transcription start. The binding of Fur or RcsAB to the hmsT promoter regions would block the entry of the RNA polymerase to repress the hmsT transcription. In addition, no change in the transcription of hmsHFRS or YPO0450-0448 was observed in the fur mutant compared to its parent strain, indicating that Fur had no regulatory activity on hmsHFRS and YPO0450-0448.
Since the genomic regions encoding Fur, HmsT, HmsHFRS, and YPO0450-0448 were extremely conserved between Y. pestis and typical Y. pseudotuberculosis [32], the regulatory circuit determined herein could be applied to Y. pseudotuberculosis. The action of at least three anti-biofilm factors NghA, RcsAB, and Fur will bring a tight biofilm-negative phenotype of typical Y. pseudotuberculosis. In contrast, Y. pestis has undergone the evolution of loss-of-function of NghA [33] and RcsA [9], which will confer a selective advantage to the progenitor Y. pestis. The mutational loss of function of Fur is of virtual impossibility, since Fur is a predominant regulator of iron assimilation in Y. pestis [13,14]. Fur-mediated repression of hmsT expression and c-di-GMP synthesis would greatly contribute to finely modulate Yesinia biofilm production within the physiological range. Moreover, Y. pestis has acquired an additional factor Ymt that promotes the bacterial survival of in fleas [30]. The above evolutionary events make Y. pestis prerequisitely survive in fleas and moreover synthesize adhesive biofilms in flea proventriculus to make the blockage, resulting in an efficient arthropod-borne transmission [34].  An oligonucleotide primer was designed to be complementary to the RNA transcript of YPO0450. The primer extension products were analyzed with 8 M urea-6% acrylamide sequencing gel. Lanes C, T, A, and G represented the Sanger sequencing reactions. Two closely neighboring extension products were detected. Only the longer product was chosen for identifying the transcription start site shown with the arrow, due to the facts that the shorter extension product might represent the premature stops resulted from the difficulty of polymerase in passing difficult nucleotide sites, and that the core promoter 235 element could not be predicted for the shorter extension product. b) LacZ fusion. A promoter-proximal region of YPO0450 was cloned into the lacZ transcriptional fusion vector pRW50, and transformed into WT or Dfur to determine the YPO0450 promoter activity (Miller units) in the cellular extracts. e) Promoter structure. Shown were translation/transcription starts, SD sequences, promoter 210 and 235 elements, and RcsAB box-like sequence for YPO0450. doi:10.1371/journal.pone.0052392.g004