Heat Shock Protein DnaJ in Pseudomonas aeruginosa Affects Biofilm Formation via Pyocyanin Production

Heat shock proteins (HSPs) play important biological roles, and they are implicated in bacterial response to environmental stresses and in pathogenesis of infection. The role of HSPs in P. aeruginosa, however, remains to be fully elucidated. Here, we report the unique role of HSP DnaJ in biofilm formation and pathogenicity in P. aeruginosa. A dnaJ mutant produced hardly any pyocyanin and formed significantly less biofilms, which contributed to decreased pathogenicity as demonstrated by reduced mortality rate in a Drosophila melanogaster infection model. The reduced pyocyanin production in the dnaJ mutant was a result of the decreased transcription of phenazine synthesis operons including phzA1, phzA2, phzS, and phzM. The reduction of biofilm formation and initial adhesion in the dnaJ mutant could be reversed by exogenously added pyocyanin or extracellular DNA (eDNA). Consistent with such observations, absence of dnaJ significantly reduced the release of eDNA in P. aeruginosa and addition of exogenous pyocyanin could restore eDNA release. These results indicate dnaJ mutation caused reduced pyocyanin production, which in turn caused the decreased eDNA, resulting in decreased biofilm formation. DnaJ is required for pyocyanin production and full virulence in P. aeruginosa; it affects biofilm formation and initial adhesion via pyocyanin, inducing eDNA release.


Introduction
Heat shock proteins (HSPs) were originally reported to recognize consensus DNA binding sites and activate genes encoding protein chaperones in response to elevated temperatures [1]. However, it has become apparent that HSPs participate in gene regulation not only by protecting cellular proteins from environmental stress but also by maintaining a cellular protein homeostasis [2]. HSPs can be divided into six main families according to their molecular weight: HSP100, HSP90, HSP70, HSP60, HSP40 and small heat shock proteins [3]. DnaJ is a typical member of the HSP40 family, and acts as a co-chaperone for HSP70 proteins, which are referred to as master players in protein homeostasis [4,5]. DnaK has been to be a DnaJ interaction partner in many bacteria. DnaJ promotes the release of substrates by promoting the transfer of substrates and stimulating the ATPase activity of its co-chaperone DnaK [6]. DnaJ, together with DnaK and DnaE, can act on the entire Escherichia coli proteome because most proteins contain multiple DnaK and DnaJ binding sites [7]. There is also increasing evidence that

Production of Pyocyanin was Drastically Reduced in the Absence of dnaJ
PYO is a critical virulence factor secreted by P. aeruginosa. It was noticed that the dnaJ-M culture had significantly decreased pigment; therefore, the production of pyocyanin in P. aeruginosa in the absence of dnaJ was measured. The results showed that the mutant produced hardly any PYO, with the level only slightly above the control. Numerically, the wild type produced eight times more PYO than the dnaJ mutant ( Figure 2a).   Growth comparison in LB broth; (b) Survival after heat shock and H2O2 treatment. Heat shock was carried out at 50 °C and 60 °C for 1 min, and H2O2 treatment with the final concentration at 0.1% for 1 min. Serial dilutions are shown underneath the images. Untreated was used as a control. The results shown are representative of three independent experiments with similar results.

Production of Pyocyanin was Drastically Reduced in the Absence of dnaJ
PYO is a critical virulence factor secreted by P. aeruginosa. It was noticed that the dnaJ-M culture had significantly decreased pigment; therefore, the production of pyocyanin in P. aeruginosa in the absence of dnaJ was measured. The results showed that the mutant produced hardly any PYO, with the level only slightly above the control. Numerically, the wild type produced eight times more PYO than the dnaJ mutant ( Figure 2a).  The expression of phzM, phzS, phzA1 and phzA2 using p-lux promoter-reporter systems in the wild-type (black) and the dnaJ-M (white) strains. The values are presented as cps normalized to OD 600 . Data shown are averages from triplicate experiments ± standard errors. A two-tailed unpaired t-test was performed using GraphPad software version 5.0 (** p < 0.01; *** p < 0.001). The results shown are representative of three independent experiments with similar results.
In P. aeruginosa, phenazine compounds are synthesized by enzymes encoded in several operons. To address the underlying mechanism of the PYO reduction in the dnaJ mutant, we first examined the transcriptional levels of the genes associated with phenazine synthesis. The results showed that the expression of phzM and phzS, which encode putative phenazine-specific methyltransferase and flavin-containing monooxygenase, respectively (enzymes which control the synthesis of PYO from phenazine-1-carboxylic acid (PCA)), was reduced fivefold and twofold respectively (Figure 2b). In addition, the expression of the phzA1 and phzA2 operons was also decreased 1.7-fold and fivefold in the dnaJ mutant compared with the wild type ( Figure 2b). This result indicates that all the operons associated with phenazine synthesis tested showed significantly decreased expression in the mutant type when compared with the wild type, which demonst rates that DnaJ affected PYO production at the transcriptional level.

The dnaJ Mutation Impaired Biofilm Formation
As PYO is involved in biofilm formation [24], we tested the biofilm formation of the dnaJ mutant. Both the initial stage of adhesion during biofilm formation and the final amount of biofilm formed were compared between the wild type and the dnaJ mutant. As shown in Figure 3a,b, both adhesion and final biofilm formation were significantly decreased in the mutant, indicating an important role for DnaJ in biofilm formation in P. aeruginosa.  The images were captured using a LAS-3000 imager system. EV: Empty vector control. p-dnaJ: dnaJ complementation construct. A two-tailed unpaired t-test was performed using GraphPad software version 5.0 (***, p < 0.001). NS: Not Significant.

The Full Pathogenicity of P. Aeruginosa Requires Functional dnaJ
The finding that DnaJ affected PYO production and biofilm formation prompted us to investigate the pathogenicity of the dnaJ mutant. The in vivo pathogenicity of the dnaJ mutant was compared with that of the wild type using a Drosophila melanogaster feeding infection model. As shown in Figure 4, the survival rate of the fruit flies fed with the dnaJ mutant was significantly higher compared with those infected with the wild type. Apparently, the full pathogenicity of P. aeruginosa The images were captured using a LAS-3000 imager system. EV: Empty vector control. p-dnaJ: dnaJ complementation construct. A two-tailed unpaired t-test was performed using GraphPad software version 5.0 (* p < 0.05; ** p < 0.01). NS: Not Significant.
Since motilities play a role in biofilm formation, we further examined the effect of dnaJ disruption on P. aeruginosa motilities. While the twitching motility was not affected (data not shown), both swarming and swimming motilities were decreased in the dnaJ mutant ( Figure 3c). The decreased swarming motility was somewhat unexpected, considering the decreased biofilm formation in the mutant. It is known that swarming motility is inversely correlated with biofilm formation in P. aeruginosa [25]. Since biofilm formation is modulated by multiple factors, the effect of motility was likely veiled by other effects of DnaJ.

The Full Pathogenicity of P. aeruginosa Requires Functional dnaJ
The finding that DnaJ affected PYO production and biofilm formation prompted us to investigate the pathogenicity of the dnaJ mutant. The in vivo pathogenicity of the dnaJ mutant was compared with that of the wild type using a Drosophila melanogaster feeding infection model. As shown in Figure 4, the survival rate of the fruit flies fed with the dnaJ mutant was significantly higher compared with those infected with the wild type. Apparently, the full pathogenicity of P. aeruginosa requires functional dnaJ. the production of biofilms in these strains; (c) the changed swarming and swimming motilities in dnaJ-M. The images were captured using a LAS-3000 imager system. EV: Empty vector control. p-dnaJ: dnaJ complementation construct. A two-tailed unpaired t-test was performed using GraphPad software version 5.0 (***, p < 0.001). NS: Not Significant.

The Full Pathogenicity of P. Aeruginosa Requires Functional dnaJ
The finding that DnaJ affected PYO production and biofilm formation prompted us to investigate the pathogenicity of the dnaJ mutant. The in vivo pathogenicity of the dnaJ mutant was compared with that of the wild type using a Drosophila melanogaster feeding infection model. As shown in Figure 4, the survival rate of the fruit flies fed with the dnaJ mutant was significantly higher compared with those infected with the wild type. Apparently, the full pathogenicity of P. aeruginosa requires functional dnaJ.

The Effect of dnaJ on Biofilm Formation Was through PYO and eDNA
Previous studies have shown that PYO can promote eDNA release in P. aeruginosa and that eDNA is a major component of biofilms [26]. Because the production of PYO was significantly decreased in the dnaJ mutant, we suspected that the changed biofilm production and adhesion in the dnaJ mutant could be due to decreased production of eDNA. The eDNA was therefore isolated directly from the cultures of the wild type and the dnaJ mutant, and the eDNA amounts were measured and compared. The results show that the dnaJ mutant produced much less eDNA compared with the wild type and the complementary strain (Figure 5a).
To confirm that the lessened eDNA in the dnaJ mutant was due to the reduced PYO observed in our experiments, we measured the amount of eDNA in supernatants of the dnaJ mutant grown with exogenously added PYO. The result showed that eDNA release was restored to the wild type level by the exogenous PYO ( Figure 5a). Consistently, biofilm formation and adhesion in the dnaJ mutant were also restored by addition of PYO (Figure 5b,c). Similarly, addition of eDNA isolated from the cultures was also able to restore biofilm formation and adhesion. These results confirm that the reduced biofilm formation and initial adhesion by the dnaJ mutant was due to the decreased PYO and subsequently reduced eDNA.
Previous studies have shown that PYO can promote eDNA release in P. aeruginosa and that eDNA is a major component of biofilms [26]. Because the production of PYO was significantly decreased in the dnaJ mutant, we suspected that the changed biofilm production and adhesion in the dnaJ mutant could be due to decreased production of eDNA. The eDNA was therefore isolated directly from the cultures of the wild type and the dnaJ mutant, and the eDNA amounts were measured and compared. The results show that the dnaJ mutant produced much less eDNA compared with the wild type and the complementary strain (Figure 5a). The initial adhesion and (c) biofilm formation in WT, dnaJ-M and dnaJ-M with exogenous eDNA at 2 µ g/mL (final concentration) or pyocyanin at 10 µ g/mL Averages of triplicate experiments ± standard errors of the means are shown. A two-tailed unpaired t-test was performed using GraphPad software version 5.0 (*, p < 0.05; **, p < 0.01; ***, p < 0.001). EV: empty vector control. p-dnaJ: dnaJ complementation construct.
To confirm that the lessened eDNA in the dnaJ mutant was due to the reduced PYO observed in our experiments, we measured the amount of eDNA in supernatants of the dnaJ mutant grown with exogenously added PYO. The result showed that eDNA release was restored to the wild type level by the exogenous PYO ( Figure 5a). Consistently, biofilm formation and adhesion in the dnaJ mutant were also restored by addition of PYO (Figures 5b,c). Similarly, addition of eDNA isolated from the cultures was also able to restore biofilm formation and adhesion. These results confirm that the reduced biofilm formation and initial adhesion by the dnaJ mutant was due to the decreased PYO and subsequently reduced eDNA. A two-tailed unpaired t-test was performed using GraphPad software version 5.0 (* p < 0.05; ** p < 0.01; *** p < 0.001). EV: empty vector control. p-dnaJ: dnaJ complementation construct.

DnaJ Affected the Production of PYO through QS Pathways
To address the underlying mechanism of PYO reduction in the dnaJ mutant, we examined the QS regulatory systems that play a crucial role in the production of PYO [27]. The expression of the QS genes was measured using the lux-based reporter system. The results obtained indicate that, except lasR, all the QS-associated genes tested, including lasI rhlR rhlI and pqsA, were downregulated in the dnaJ mutant (Figure 6a). Consistent with this observation, significantly fewer PQS signals were detected in the dnaJ mutant (Figure 6b). These results suggest that DnaJ affected the production of PYO through both the AHL-and PQS-based QS pathways.
QS regulatory systems that play a crucial role in the production of PYO [27]. The expression of the QS genes was measured using the lux-based reporter system. The results obtained indicate that, except lasR, all the QS-associated genes tested, including lasI rhlR rhlI and pqsA, were downregulated in the dnaJ mutant (Figure 6a). Consistent with this observation, significantly fewer PQS signals were detected in the dnaJ mutant (Figure 6b). These results suggest that DnaJ affected the production of PYO through both the AHL-and PQS-based QS pathways.

Discussion
HSP genes are highly conserved in all eukaryotes and prokaryotes, and they participate in a number of fundamental cellular processes such as controlling protein folding and gene expression. Interestingly, some HSPs have been identified as virulence factors, while others are involved in pathogenesis indirectly [9]. P. aeruginosa is an important human pathogen that causes serious infections, especially in patients with underlying medical conditions or immunocompromised patients. The data obtained in this study indicate that the inactivation of dnaJ in P. aeruginosa caused a dramatic reduction in PYO production, decreased adherence and biofilm formation. HSP DnaJ in P. aeruginosa seems to have a significant effect on the pathogenicity of P. aeruginosa.
HSPs are important for bacterial survival and adaptation to adverse environmental conditions. Previous studies have shown that the absence of djlA, a member of the same DnaJ family as Legionella dumoffii [28] and Streptococcus suis type 2, can affect bacterial growth [29], but the mutation of dnaJ of P. aeruginosa has no effect on bacterial growth (Figure 1a). The cells of the dnaJ mutant treated with heat shock and H2O2 had a similar survival rate to the wild type cells. It is possible that P. aeruginosa has other HSPs that could compensate the loss of dnaJ. For instance, P. aeruginosa has cbpA on its chromosome; this is a dnaJ homolog that has a similar function to dnaJ in cell growth and division in E. coli [6]. Two-tailed unpaired t-test was performed using GraphPad software version 5.0 (* p < 0.05; ** p < 0.01; *** p < 0.001). NS: Not Significant. (b) Comparison of PQS production between the WT and dnaJ-M. PQS in the cultures was isolated and analyzed on high performance thin layer chromatography (TLC). Extract from 500 µL of culture equivalent was loaded onto the TLC plate.

Discussion
HSP genes are highly conserved in all eukaryotes and prokaryotes, and they participate in a number of fundamental cellular processes such as controlling protein folding and gene expression. Interestingly, some HSPs have been identified as virulence factors, while others are involved in pathogenesis indirectly [9]. P. aeruginosa is an important human pathogen that causes serious infections, especially in patients with underlying medical conditions or immunocompromised patients. The data obtained in this study indicate that the inactivation of dnaJ in P. aeruginosa caused a dramatic reduction in PYO production, decreased adherence and biofilm formation. HSP DnaJ in P. aeruginosa seems to have a significant effect on the pathogenicity of P. aeruginosa.
HSPs are important for bacterial survival and adaptation to adverse environmental conditions. Previous studies have shown that the absence of djlA, a member of the same DnaJ family as Legionella dumoffii [28] and Streptococcus suis type 2, can affect bacterial growth [29], but the mutation of dnaJ of P. aeruginosa has no effect on bacterial growth (Figure 1a). The cells of the dnaJ mutant treated with heat shock and H 2 O 2 had a similar survival rate to the wild type cells. It is possible that P. aeruginosa has other HSPs that could compensate the loss of dnaJ. For instance, P. aeruginosa has cbpA on its chromosome; this is a dnaJ homolog that has a similar function to dnaJ in cell growth and division in E. coli [6].
The most obvious change in the P. aeruginosa dnaJ mutant was its diminished PYO production. P. aeruginosa has the ability to produce pigmented secondary metabolites including PYO and several other phenazine compounds. PYO is a critical virulence factor in P. aeruginosa during chronic infection [30]. It appears that the reduction of PYO production was mediated by the downregulation of phzM, phzS, and the phzA1 and phzA2 operons. Therefore, DnaJ may affect PYO production by directly regulating the phz genes. However, it is well known that QS systems control the production of PYO in P. aeruginosa; this points to an indirect route where DnaJ could assert its effect on PYO production. The reduced expression of QS-related genes, such as lasI, rhlR, rhlI, and pqsA, in the dnaJ mutant seems to indicate that the DnaJ indirectly affects PYO production through the QS systems. The comparison of PQS in the P. aeruginosa wild type and dnaJ mutant cultures confirms the effect of DnaJ on the QS systems.
Biofilm formation is an important characteristic during P. aeruginosa chronic infection. Bacterial cells in biofilms are protected from antimicrobial drugs and the host immune response. Both initial adhesion and final biofilm formation in the dnaJ mutant were significantly decreased. Multiple factors could have contributed to such a reduction in biofilm formation. PYO can promote extracellular DNA (eDNA) release in P. aeruginosa and eDNA is essential for biofilm formation [26]. We detected the production of eDNA in the LB and Pseudomonas broth (PB) media with or without exogenous PYO. The results confirmed that the reduced production of eDNA was, at least partially, due to the loss of PYO production. Previous literature has also shown that a pqsA mutant, deficient in the production of PQS, released low amounts of extracellular DNA, and a pqsL mutant, which overproduces PQS, released large amounts of extracellular DNA [31]. Therefore, the decreased eDNA in the dnaJ mutant could also be due to the decreased PQS caused by the absence of dnaJ.
Both PYO and biofilms play an important role in the pathogenicity of P. aeruginosa. The effect of dnaJ on the in vivo pathogenicity of P. aeruginosa was confirmed by the fruit fly infection assay. The mutant-strain-fed flies had better survival rates than the wild-type-fed flies. However, it is noted that the effect of dnaJ could be through virulence-related pathways other than PYO and biofilm formation. It is possible that other virulence factors not tested in our study could also been affected by the disruption of dnaJ. After all, DnaJ as a chaperon protein could interact with many virulence-associated or non-virulence-associated proteins. It has been reported that nearly all the proteins in the E. coli proteome are predicted to contain multiple DnaK-and DnaJ-binding sites [7]. Therefore, the effect of DnaJ on pathogenicity in P. aeruginosa may be multifactorial. Nevertheless, the requirement of DnaJ for the full pathogenicity of P. aeruginosa appears quite clear.
The flagella-propelled swimming and swarming motilities of P. aeruginosa are also a virulence factor in host invasion [32]. In agreement with previous studies, which show that dnaJ mutation in E. coli causes decreased flagellin synthesis [33], the defective swimming and swarming in the dnaJ mutant of P. aeruginosa might also be caused by defected flagellar biosynthesis. Since swarming motility is known to be related to biofilm formation, the decreased swarming motility in the dnaJ mutant seems to contradict the reduced biofilm formation and reduced initial adhesion observed. Decreased motility would promote biofilm formation, especially at the initial stages [34]. However, the reduced biofilm formation is probably a combined result of different changes in the dnaJ mutant. The effect of the decreased motility was probably concealed by other changes such decreased eDNA release, that would instead result in decreased biofilm formation.
Taken together, we reported that DnaJ, an HSP40 family protein in P. aeruginosa, contributes to the bacterium's pathogenicity. It significantly affects PYO production and biofilm formation. Further study of DnaJ and its regulation pathway should contribute to a better understanding of the pathogenesis of P. aeruginosa infection and to the exploration of new therapeutic targets.

Bacterial Strains, Culture and Media
The plasmids and strains used in this study have are listed in Table S1 and the primers used in this study are listed in Table S2. For the culture media, Luriae Bertani (LB) medium and Pseudomonas broth (PB) (2% Peptone, 0.14% MgCl 2 , 1% K 2 SO 4 ), which is a medium to maximize pyocyanin production in liquid culture, were used. All strains were grown aerobically at 37 • C. The antibiotics used in this study were as follows. For Escherichia coli, Gentamicin (Gm, 15 µg/mL), Kanamycin (Kn, 50 µg/mL) and ampicillin (Amp, 100 µg/mL) were used. For P. aeruginosa, carbenicillin (Cb, 500 µg/mL) and trimethoprim (Tmp, 300 µg/mL) were used. All antibiotics were purchased from MP Biomedicals, LLC (Solon, OH, USA) and other chemicals were purchased from the Tianjin Kemiou Chemical Reagent Co., Ltd. (Tianjin, China).

Bacterial Survival Test by Growth Assay
The growth of each strain was measured using the microplate reader and colony-forming units (CFU). The cells were cultured overnight at 37 • C and 200 rpm after inoculation in fresh LB broth. The bacterial solution was adjusted from OD 600 to 0.01, and then the growth was measured in 96-well plates using the microplate reader according to a 5% inoculation. In addition, the strains cultivated in 5 mL LB overnight were adjusted to OD 600 = 0.5, and a serious of dilutions from 10 −1 to 10 −7 were made. Each dilution gradient was placed 5 µL on an LB plate and then incubated for 16 h. The experiment was repeated at least three times.

Motility Assays
The motility assay was carried out as described previously with minor modifications [35]. The swarming motility medium comprised 0.8% nutrient broth, 0.5% glucose and 0.5% agar. The swimming medium comprised 1% tryptone, 0.5% sodium chloride and 0.3% agar. Plates were dried at room temperature overnight before being used. The 2 µL bacterial solution was spotted onto the swimming and swarming plates. After the solution was completely inhaled into the medium, they were carefully removed to a 37 • C incubator for 24 h. Photographs were taken with the LAS-3000 imaging system (Fuji Corp). The experiment was repeated at least three times.

Measurement of PYO Production
Pyocyanin was extracted from culture supernatants and measured using previously reported methods [36]. Briefly, the cells were cultured for 18 h in PB medium at 37 • C and 3 mL chloroform was added to 5 mL culture supernatant. After extraction, the chloroform layer was transferred to a fresh tube and mixed with 1 mL 0.2 M HCl. After centrifugation, the top layer (0.2 M HCl) was removed and its A520 was measured. The amount of pyocyanin, in µg/mL, was calculated using the following formula: A520/A600 × 17.072 = µg of pyocyanin per mL.

Monitoring Gene Expression by Lux-Based Reporters
The reporter strains (named pMS402) carry a promoterless luxCDABE reporter gene cluster (p-lux reporter system). The promoter region of the target genes was amplified by PCR, and the PCR products were digested by BamHI-XhoI. The enzyme-digested products were cloned into pMS402. The expression of these genes was monitored using light production Luminescent lux reporter strains in 96-well microtiter plates as reported previously with minus modification [37]. Briefly, strains containing different reporters were cultivated overnight in LB broth supplemented with Tmp (300 µg/mL). Overnight cultures of the reporter strains were diluted to an optical density at 600 nm (OD 600 ) of 0.2 and cultivated for an additional 2 h before use as inoculants. Aliquots of a fresh culture (5 µL) were inoculated into parallel wells on a 96-well black plate with a transparent bottom, which contained 95 µL of medium with Tmp (300 µg/mL). To prevent evaporation during the assay, 70 µL of filter-sterilized mineral oil was added. Both luminescence and bacterial growth (OD 600 ) were measured every 30 min for 24 h in a BioTek Synergy 2 plate reader, and data were collected using Gen5 software. The level of light production, measured in counts per second (cps), was proportional to the level of gene expression. The light production values were then normalized to the level of bacterial growth. The level of gene expression is presented as the number of relative expressions, calculated as cps/OD 600 by use of the normalized cps values.

Quantification of Initial Adhesion and Biofilm Formation
The initial adhesion and biofilm production were measured in a static system, as previously described [38], with minor modifications. Quantification of the initial adhesion was carried out in 15 mL borosilicate tubes. Briefly, cells from overnight cultures were inoculated at 1:100 dilutions into PB media and statically grown at 37 • C for 8 h. For the biofilm production, strains were grown at 37 • C for at least 24 h. After removing the bacterial solution, the test tube was stained by 1% crystal violet for 20 min, and 1mL 95% ethanol was used to dissolve the crystal violet. The solution was measured at 600 nm. The experiment was repeated at least three times.

In Vivo Pathogenicity Assay Using Drosophila Melanogaster Feeding Infection Model
The fly-feeding assay was applied as previously reported [39]. For infection, 1.0 mL of the culture, which was adjusted to OD 600 = 2.0 using the media the strain was grown in, was collected by centrifugation. The supernatant was then removed and the resulting pellet was resuspended in 100 mL of 5% sucrose. Then, 100 µL 0.1 M sucrose solution and the same amount of bacterial solution were added to filter paper, which was placed on the surface of 2 mL of solidified 0.1 M sucrose agar in a 20 mL glass tube with silica gel stopper. Male flies (3-5 days old) were starved for 3 h before 10 flies were added to each tube. A cold shock method was used for anesthetizing flies throughout the sorting and transferring process. Infection tubes were stored at 26 • C in a humidity-controlled environment. The number of live flies at the start of the experiment was documented, and live flies were counted at 24 h intervals for 6 days. Survival percent was determined for groups of 60 drosophila flies (with 6 batches of 10 flies per vial) at 26 • C.

eDNA Assay
The cells were cultured in 5 mL PB for overnight at 37 • C 200 rpm. The cells from overnight cultures were separated by centrifugation at 6000× g for 10 min at 4 • C. After the supernatant was filtered, the cell-free supernatant (3 mL) was used for DNA recovery following the instructions of the DNA gel extraction kit, which are as follows. Briefly, add 1 volumes of buffer to 1 volume of supernatant. To bind DNA, apply the sample to the column and then centrifuge for 1 min. For sample volumes > 800 µL, simply load the remainder and spin again. To wash, add 0.75 mL of washing buffer into the column and centrifuge for 1 min (repeat once). Discard the flow-through and centrifuge the column for an additional 1 min at 7900× g. To elute DNA, add 50 µL of buffer EB (10 mM Tris-Cl, pH 8.5) to the center of the membrane, and then centrifuge the column for 1 min. The purified eDNA (15 µL) mixed with the loading buffer is then to be analyzed on a gel. After completing the process, the gel was visualized using the Syngene GeneGenius Bio Imaging System (Synoptics Ltd, Cambridge, UK). The experiment was repeated at least three times.

PQS Extraction and Quantification
Each strain was grown in PB broth for 24 h, and then the cells of supernatant were removed by centrifugation at 20,000× g for 5 min, and the supernatant was filtered through a polytetrafluoroethylene membrane (pore size, 0.22 µm). Aliquots of culture supernatants were subjected to two extractions by addition of one volume of acidified ethyl acetate (0.01% acetic acid). The organic phase was transferred to a fresh tube and dried to completion. The solutes were re-suspended in methanol for TLC analysis. The sample was spotted onto a TLC plate which had been previously soaked for 30 min in 5% KH 2 PO 4 and activated at 100 • C for 1 h. Extracts (PQS) were separated using a dichloromethane: methanol (95:5) system until the solvent front reached the top of the plate. The plate was visualized using a UV and photographed. Standard QS signals were used as a positive control. The experiment was repeated at least three times.

Statistical Analysis
All statistical analyses were performed using GraphPad Prism version 5 (GraphPad Software, La Jolla, CA, USA). The two-tailed unpaired t-test was used to analyze the data. * p < 0.05; ** p < 0.01; *** p < 0.001. Values are expressed as mean ± standard errors of the means.