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Microarray Analysis Reveals Induction of Lipoprotein Genes in Mucoid Pseudomonas aeruginosa: Implications for Inflammation in Cystic Fibrosis

Department of Molecular Genetics and Microbiology, University of New Mexico Health Sciences Center, Albuquerque, New Mexico

Received 13 January 2004/ Returned for modification 25 February 2004/ Accepted 8 June 2004

	ABSTRACT

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The main cause of the high morbidity and mortality of cystic fibrosis (CF) is the progressive lung inflammation associated with Pseudomonas aeruginosa colonization. During the course of chronic CF infections, P. aeruginosa undergoes a conversion to a mucoid phenotype. The emergence of mucoid P. aeruginosa in CF is associated with increased inflammation, respiratory decline, and a poor prognosis. Here we show, by the use of microarray analysis, that upon P. aeruginosa conversion to mucoidy, there is a massive and preferential induction of genes encoding bacterial lipoproteins. Bacterial lipoproteins are potent agonists of Toll-like receptor 2 (TLR2) signaling. The expression of TLR2 in human respiratory epithelial cells was ascertained by Western blot analysis. Human respiratory epithelial cells responded in a TLR2-dependent manner to bacterial lipopeptides derived from Pseudomonas lipoproteins induced in mucoid strains. The TLR2 proinflammatory response was further augmented in CF cells. Thus, the excessive inflammation in CF is the result of a global induction in mucoid P. aeruginosa of lipoproteins that act as proinflammatory toxins (here termed lipotoxins) superimposed on the hyperexcitability of CF cells. Blocking the signaling cascade responding to bacterial lipotoxins may provide therapeutic benefits for CF patients.

	INTRODUCTION

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Cystic fibrosis (CF) is the most common lethal inheritable disease affecting Caucasians (19). CF is caused by mutations in the gene encoding cystic fibrosis transmembrane conductance regulator (CFTR), resulting in multiorgan malfunctions, particularly within the respiratory, gastrointestinal, hepatobiliary, and reproductive tracts (29, 44). The lung complications in CF include chronic respiratory infections, which are the main cause of CF remaining an incurable lethal disease (15). The predominant CF pathogen is Pseudomonas aeruginosa: the lungs of >90% of all CF patients eventually become colonized with this bacterium (11). A classical feature of P. aeruginosa strains infecting CF patients is that they mutate into a mucoid, exopolysaccharide alginate-overproducing form in a process referred to as the conversion to mucoidy (15). The conversion to mucoidy is concomitant with the establishment of chronic bacterial colonization (20, 27). Infections with mucoid P. aeruginosa are associated with heightened inflammation, tissue destruction, and pulmonary function decline (3). It has been recognized that the establishment of mucoid P. aeruginosa biofilms correlates with a poor prognosis for CF patients (11, 20, 27). Conversion to mucoidy results from mutations that render the P. aeruginosa stress response sigma factor AlgU constitutively active (21, 22). This in turn activates genes of the alginate biosynthesis pathway and additional genes that still need to be fully characterized (9, 10).

However, the overproduction of alginate, an immunologically inert exopolysaccharide associated with mucoid conversion, cannot explain the increased inflammation in CF. This makes it likely that additional, less conspicuous, but potentially more damaging products of P. aeruginosa are produced by mucoid P. aeruginosa in the CF host. Here we describe the previously unappreciated induction of proinflammatory products in mucoid P. aeruginosa and how they affect signaling pathways in host respiratory cells. Using microarray analysis, we found that the most prominently induced genes in mucoid P. aeruginosa encode lipoproteins. We show that these P. aeruginosa products cause the activation of NF-B in human lung epithelial cells and that this occurs through Toll-like receptor 2 (TLR2).

	MATERIALS AND METHODS

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Bacterial strains and growth conditions. The mucoid P. aeruginosa strain PAO578II (mucA22 sup-2) and its isogenic nonmucoid PAO6865 (algU::Tc^r) derivative have been described previously (7). For RNA isolation, strains were cultured at 37°C overnight in Luria broth. One milliliter of the overnight culture was used to inoculate 100 ml of Luria broth containing 0.3 M NaCl, and the culture was grown for 4 h at 37°C to mid-log phase (optical density at 600 nm of 0.5).

Microarray analysis. For microarray analysis and primer extension, RNAs were isolated with Trizol (Invitrogen Life Technologies, Carlsbad, Calif.) and an RNeasy kit (Qiagen, Valencia, Calif.) according to the method described by Lory et al. (http://cfgenomics.unc.edu/protocols_rna_prep.htm). Labeled cDNAs were generated according to the protocol for the Affymetrix (Santa Clara, Calif.) Pseudomonas microarray chip. cDNAs were synthesized by annealing random primers (Invitrogen) to purified RNAs and extending them with SuperScript II (Invitrogen). Transcripts corresponding to Bacillus subtilis genes dap, thr, phe, lys, and trp were spiked into the cDNA synthesis reaction mixtures as a control to monitor cDNA synthesis, labeling, hybridization, and staining efficiency (courtesy of Steve Lory, Harvard Medical School). RNAs were removed by the addition of 1 N NaOH and incubation at 65°C for 30 min. The reaction was neutralized with 1 N HCl, and the cDNAs were purified with a Qiaquick PCR purification kit (Qiagen). The yields were quantified, and cDNAs were fragmented with 0.6 U of DNase I (Amersham Pharmacia Biotech) per µg of cDNA for 10 min at 37°C, followed by heat inactivation. Chips were hybridized overnight at 50°C and then washed, stained, and scanned the next day according to the steps of the Affymetrix Microarray Suite software specified for the Pseudomonas chip. The results from three independent experiments were merged for each strain. The merged data were used for comparisons, and statistical significance was assessed with Student's t test.

Cell culture. Primary normal human bronchial epithelial cells (NHBEs) (Cambrex Bio Science, Baltimore, Md.) were cultured in bronchial epithelial medium (BEGM; Cambrex Bio Science). IB3-1 (47) is a CF-affected human airway epithelial cell line. Genotypically, IB3-1 is a compound heterozygote containing the F508 mutation and W1282X. The C38 and S9 cell lines, created by correcting IB3-1 cells for chloride conductance by the introduction of functional CFTR (8), were grown in LHC-8 medium (Bio-fluids, Rockville, Md.) supplemented with 10% fetal bovine serum and antibiotics. S9 and C38 cells are both functionally complemented for the major known CFTR effects. They differ in that the CFTR cDNA used to complement IB3-1 cells encodes a complete CFTR molecule in the case of S9 cells, while it lacks the first CFTR extracellular loop in the case of C38 cells (47). NuLi-1 cells, derived from normal human airway epithelial cells by J. Zabner (46), were cultured in collagen-coated plastic dishes (Sigma, St. Louis, Mo.) in serum-free bronchial epithelial cell growth medium with supplements (Clonetics/BioWhittaker, San Diego, Calif.). The 9/HTEo^– tracheal epithelial cell line (28), obtained from P. Davis (Case Western Reserve University, Cleveland, Ohio), was maintained in Dulbecco's modified Eagle's medium supplemented with 10% fetal bovine serum and 2.5 mM L-glutamine (in the presence of 50 U of hygromycin/ml as a marker of the cell line due to its stable transfection with the pCEP2 vector). All cell lines were grown at 37°C in 5% CO₂. For luciferase and cytokine assays, cells were seeded at 5 x 10⁵ or 1 x 10⁵ cells/well in 12-well plates, respectively.

Peptide design and synthesis. Leader sequences denoting lipopeptide modification (31) were observed for two open reading frames (ORFs) downstream of AlgU-dependent promoters. Two peptides, LPTA(6) (Pam₃Cys-DKKEE-OH) and LPTB(6) (Pam₃Cys-DSQTN-OH), consisting of a palmitylated cysteine (Pam₃Cys) after the cleavage site plus five amino acids from the amino terminus of each lipoprotein, were synthesized (Bio-Synthesis, Inc., Lewisville, Tex.). The proinflammatory synthetic bacterial lipopeptide Pam₃Cys-SKKKK-OH was also synthesized (2, 17).

Transfection, luciferase reporter, and cytokine assays. To monitor transient NF-B activation, we seeded the primary NHBE, IB3-1, C38, and S9 cell lines at 5 x 10⁵ cells per well in a 12-well plate and transfected them by using the Effectene transfection reagent (Qiagen) with 0.05 µg of a human TLR2 (hTLR2) or dominant-negative TLR2 (DN-TLR2) expression plasmid, 0.15 µg of an NF-B-responsive luciferase reporter construct, 0.15 µg of a control Renilla luciferase construct, and 0.05 µg of a control ß-galactosidase reporter construct for normalization. Eighteen hours after transfection, the cells were incubated with a stimulus (tumor necrosis factor alpha [TNF-], 20 ng/ml; lipopolysaccharide [LPS], 1 µg/ml; Pam₃Cys, 5 µg/ml; or lipopeptides, 5 µg/ml) for 6 h and assayed for luciferase activity by use of a luciferase assay reagent (Promega) or for ß-galactosidase activity by use of the Galacto-Star luminescence system (Tropix, Bedford, Mass.). The transfection efficiency was controlled by standardizing the luciferase activity to constitutive ß-galactosidase production. For the cytokine assay, NHBE confluent monolayers were incubated with LPS (1 µg/ml), bacterial lipopeptides (1 or 10 µg/ml), or no stimulation for 24 h. Cell culture supernatants were assayed at a 100-fold dilution for secreted interleukin-8 (IL-8) according to the manufacturer's instructions (R&D Systems, Minneapolis, Minn.). All experiments were repeated at least three times, and all errors shown represent experimental errors for at least three independent cultures.

Western blot analysis and antibodies. Protein samples were prepared by homogenizing lung epithelial cells in lysis buffer (8.5% sucrose and protease inhibitors [10 mg of leupeptin/ml, 1 µM pepstatin, 1.8 mg of E64/ml, and 5 mg of N-p-tosyl-L-lysine chloromethyl ketone/ml]) (all chemicals were from Sigma Chemical Co.) on ice. Protein concentrations were determined by the use of a micro BCA protein assay reagent kit (Pierce, Rockford, Ill.). An antibody against TLR2 for Western blotting was obtained from Imgenex (San Diego, Calif.). Immune complexes were detected with horseradish peroxidase-conjugated goat anti-mouse immunoglobulin G (Bio-Rad, Hercules, Calif.). The signal was visualized by incubating the complexes with Super Signal chemiluminescent substrate (Pierce). Densitometric analyses of Western blots were performed with NIH Image software (http://rsb.info.nih.gov/nih-image). Western blot quantification was performed as previously described (13, 14, 43). A blocking antibody against TLR2 was obtained from Douglas Golenbock.

	RESULTS

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The most highly induced genes in mucoid P. aeruginosa encode lipoproteins. It has been shown that the conversion to mucoidy in P. aeruginosa CF isolates occurs via mutations in the mucA gene (22) that activate the alternative sigma factor AlgU (21, 22). We tested how the activation of AlgU in a mucoid P. aeruginosa strain carrying the most common mucA mutation found in CF isolates affected global gene expression. PAO578II carries the mucA22 mutation and an additional sup-2 mutation, also common among CF isolates, that renders it responsive to growth conditions for the maximal production of alginate (35). The strain PAO6865 is an algU knockout (algU::Tc^r) derivative of PAO578II (4). When the microarray expression data (Fig. 1) for PAO578II and PAO6865 were compared, the analysis revealed massive and selective lipoprotein induction in mucoid P. aeruginosa, with high expression ratios (Fig. 1, crosses, and Table 1). We found that 70% of the genes showing induction above 30-fold encoded uncharacterized lipoproteins (Table 1). The highest levels of AlgU-dependent expression were observed with the lipoprotein genes lptE and lptG. Two of the lipoprotein-encoding genes, lptA and osmE, have known AlgU-dependent promoters (10). The majority of the other highly induced genes encoding products with lipoprotein leader sequences contained an AlgU promoter consensus motif (Table 2). Since lipoproteins have been implicated in inflammatory processes and the pathogenesis of several important bacterial infections, including Mycobacterium tuberculosis (5), Treponema pallidum (40), Listeria monocytogenes (12), and Borrelia burgdorferi (32), this observation warranted further analysis.

View larger version (40K): [in this window] [in a new window]   FIG. 1. Global gene expression analysis by use of microarrays reveals massive and selective lipoprotein gene induction in mucoid P. aeruginosa. The experimental points represent merged expression data from three independent cultures run on three separate chips for each strain. Mucoid strain PAO578II carries the typical CF mutation mucA22, which causes mucoidy in P. aeruginosa. Gene expression in PAO578II was compared to that in the isogenic, nonmucoid, algU knockout strain PAO6865. Large crosses, lipoprotein genes induced in mucoid P. aeruginosa (P < 0.001). Diagonal lines delimit regions of 30-fold induction.

View this table: [in this window] [in a new window]   TABLE 2. P. aeruginosa AlgU (E) promoter consensus sequence in front of the lpt genes

P. aeruginosa lipopeptides stimulate NF-B activation in human lung epithelial cells.

View larger version (25K): [in this window] [in a new window]   FIG. 2. Lipopeptides induce inflammatory response in human respiratory epithelial cells. (A) Lipopeptides induce NF-B activation in primary human bronchial epithelial cells. NHBEs were transfected with an NF-B-responsive luciferase construct and incubated for 6 h in the presence of 1 µg of LPS/ml, 20 ng of TNF-/ml, or 5 µg of lipopeptide/ml. The data were normalized to a cotransfected ß-galactosidase construct. sBLP, synthetic bacterial lipopeptide (Pam3Cys-SKKKK-OH); LPTA(6), N terminus of lptA gene product (Pam3Cys-DKKEE-OH); LPTB(6), N terminus of lptB gene product (Pam3Cys-DSQTN-OH). (B) Western blot analysis of TLR2 protein expression in CF (IB3-1) and CFTR-corrected (C38) cells with an anti-hTLR2 monoclonal antibody (IMG-319), detected as an 86-kDa band. Equal amounts of proteins were loaded. A densitometry analysis of the TLR2 protein was performed for three independent experiments with NIH Image 1.62 software. The numbers underneath the gel represent the means ± standard errors (arbitrary density units). (C) NF-B luciferase assay with primary NHBEs showing that TLR2 activates the LPTA(6)-induced response in epithelial cells by employing DN-TLR2. *, P < 0.05; **, P < 0.01.

View larger version (20K): [in this window] [in a new window]   FIG. 3. TLR-dependent induction of NF-B-mediated transcription in bronchial epithelial cells stimulated with P. aeruginosa lipopeptide. 9/HTEo– (A) and NuLi-1 (B) cells (both derived from normal human lung cells) were transiently cotransfected with an NF-B-responsive luciferase reporter plasmid and TLR2 or DN-TLR2 and then incubated for 6 h in the presence of 10 µg of lipopeptide (LptA)/ml. The data were normalized to a cotransfected ß-galactosidase construct and are means ± standard deviations. (C) Western blot analysis of TLR2 protein expression in NuLi and 9/HTEo– cells with an anti-hTLR2 monoclonal antibody (IMG-319). Equal amounts of proteins were loaded. *, P < 0.05.

TLR2 is involved in Pseudomonas lipopeptide-induced NF-B activation in CF cells.

View larger version (34K): [in this window] [in a new window]   FIG. 4. Proinflammatory action of LptA lipopeptide in the CF bronchial epithelial cell line IB3-1 and its CFTR-corrected derivatives C38 and S9 and TLR2 dependence of the response. (A) Induction of NF-B-mediated transcription in vitro. For a luciferase assay, IB3-1, C38, and S9 cells were transiently transfected with an NF-B-responsive luciferase reporter plasmid and TLR2 or DN-TLR2 and then incubated for 6 h in the presence of 5 µg of lipopeptide/ml. The data were normalized to a cotransfected ß-galactosidase construct. (B) P. aeruginosa-based lipopeptides induce inflammatory IL-8 chemokine production by NHBEs. Confluent monolayers of NHBEs were left unstimulated (in medium) or were incubated for 24 h with P. aeruginosa LPS, 1 or 10 µg of lipopeptide/ml [sBLP, LPTA(6), or LPTB(6)], or a palmitylated cysteine control. (C) NHBEs were stimulated with LPTA(6) and LPTB(6) in the absence or presence of 20 µg of TLR2-blocking antibody (TL2.1)/ml. *, P < 0.05; **, P < 0.01.

	DISCUSSION

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The results of this study show that P. aeruginosa causes excessive inflammation in CF due to a massive and selective induction of lipoprotein genes upon conversion to mucoidy. The lipopeptides derived from such proteins show a strong proinflammatory potential in primary lung epithelial cells. In our view, these products are toxic to the CF host and thus should be considered bacterial toxins. Due to their significance in CF and their implications in pathogenesis in other infections (1, 24, 33), lipoproteins should be viewed as a double-edged sword in host-pathogen interactions: they can serve both as signals recognized by the host to activate its defenses and as agents causing excessive host damage by the pathogen in some situations, such as in CF. We have consequently designated the highest expressing lipoprotein genes in mucoid P. aeruginosa as genes encoding lipotoxins (LPTs): lptA, lptC, lptD, lptE, lptF, and lptG (Table 1).

Increased levels of IL-8 have been noted in the sputum and bronchoalveolar lavage of patients with CF (3, 34). IL-8 is known to play a major role in inflammatory pathogenesis in the airways of CF patients (3, 23, 34, 39). Synthetic lipopeptides corresponding to the N termini of the mature, processed LPTs caused IL-8 production in primary human epithelial cells, as shown here, and in human macrophages derived from peripheral blood monocytes (9). Previous studies have shown IL-8 secretion in response to P. aeruginosa in human bronchial epithelial cells (6, 7, 42), although the factors responsible have not been identified. Our results show that the primary human respiratory epithelial cells have the machinery to recognize and respond to bacterial lipoproteins and that the production of IL-8 in CF may be due to stimulation with Pseudomonas lipopeptides.

CF cells showed increased responses to lipopeptide stimulation relative to genetically matched CFTR-corrected cell lines. This indicates that CF cells can be primed for TLR2 signaling to levels that are higher than normal. Thus, both the pathogen and the host conspire to bring about excessive inflammation in CF. The differences in TLR2 responsiveness between CF and CFTR-corrected cells cannot be explained, however, by differences in the expression levels of TLR2 in CF and CFTR-corrected cells, as we did not observe any dissimilarity between IB3-1, C38, and S9 cells (Fig. 2B). Thus, it is likely that other parts of the signaling pathway downstream of or parallel to the TLR2 function differ between CF and CFTR-corrected cells. For example, recent data that were published while this study was under review suggest that TLR2 may be distributed slightly differently within plasma membrane domains in CF and normal cells (25). Furthermore, TLR2 activity may be additionally amplified in CF by asialoganglioside gangliotetraosylceramide (aGM1) (38), as aGM1 is increased in CF respiratory epithelial cells (18) due to hyperacidification of the trans-Golgi network in CF cells (29, 30). Also, note that in our experiments, transfection with DN-TLR2 did not eliminate the endogenous TLR2 response (Fig. 2C). One explanation for this observation is that the endogenous, preassembled signaling complexes responding to lipopeptides [Fig. 2C, control and LPTA(6)] may be resistant [Fig. 2C, LPTA(6) versus DN-TLR2+LPTA(6)] in respiratory epithelial cells to the superimposed expression of DN-TLR2 (defined as dominant negative in myeloid cells).

While in most challenges the TLR response may serve to limit infections, in other situations it can result in tissue destruction, as in CF and other diseases (2). The pattern recognition receptors of the host play a beneficial role in inducing innate clearance mechanisms. However, when preexisting conditions preclude smooth clearance of the invading pathogens, the same receptors may become targets for the destructive action of bacterial toxins such as LPTs, as in the case of P. aeruginosa in CF.

The microarray data and follow-up experiments presented here help to explain critical aspects of the runaway inflammatory processes in the CF lung. Other factors linked to the genetic lesion in CFTR and other modifier genes in CF patients certainly contribute to the colonization and establishment of P. aeruginosa in the lung (16). Superimposed on such preconditioned milieu, the previously unrecognized massive induction of genes encoding proinflammatory lipoproteins is likely responsible for the tissue destruction that causes high morbidity and mortality of CF patients. We envision that a simultaneous induction of a large number of lipoprotein genes may result in an additive action, although additional more complex synergisms cannot be excluded.

The knowledge of the molecular basis for the excessive inflammation in CF via bacterial lipoproteins and TLR2 may provide targets for blocking or dampening the signaling cascade, including potential applications of neutralizing or blocking antibodies, thus eliminating the factors that are ultimately responsible for respiratory failure in CF patients.

	ACKNOWLEDGMENTS

 
We thank P. Zaitlin for IB3-1, C38, and S9 cells, J. Zabner for NuLi-1 cells, P. Davis for 9HTEo^– cells, and D. Golenbock for TLR2-blocking antibodies.

Microarray instrumentation was supported by the Keck-UNM Genomics Resource core facility at the University of New Mexico. The cost of P. aeruginosa microarray chips was defrayed in part by subsidy grant 012 from the Cystic Fibrosis Foundation Therapeutics Inc. This work was supported by Philip Morris Incorporated and by NIH grants AI31139 and AI050825.

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Molecular Genetics and Microbiology, University of New Mexico Health Sciences Center, 915 Camino de Salud NE, Albuquerque, NM 87131. Phone: (515) 272-0291. Fax: (505) 272-5309. E-mail: vderetic{at}salud.unm.edu.

Editor: J. N. Weiser

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