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Pseudomonas Lipopolysaccharide Accelerates Wound Repair via Activation of a Novel Epithelial Cell Signaling Cascade¹

Jonathan L. Koff^*,, Matt X. G. Shao^*,, Suil Kim^*,, Iris F. Ueki^* and Jay A. Nadel^2,*,,

^* Cardiovascular Research Institute, Department of Medicine, and Department of Physiology, University of California, San Francisco, San Francisco, CA 94143

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
The surface of the airway epithelium represents a battleground in which the host intercepts signals from pathogens and activates epithelial defenses to combat infection. Wound repair is an essential function of the airway epithelium in response to injury in chronic airway diseases, and inhaled pathogens such as Pseudomonas bacteria are implicated in the pathobiology of several of these diseases. Because epidermal growth factor receptor (EGFR) activation stimulates wound repair and because LPS activates EGFR, we hypothesized that LPS accelerates wound repair via a surface signaling cascade that causes EGFR phosphorylation. In scrape wounds of NCI-H292 human airway epithelial cells, high concentrations of LPS were toxic and decreased wound repair. However, lower concentrations of LPS accelerated wound repair. This effect was inhibited by treatment with a selective inhibitor of EGFR phosphorylation (AG 1478) and by an EGFR neutralizing Ab. Metalloprotease inhibitors and TNF--converting enzyme (TACE) small interfering RNA inhibited wound repair, implicating TACE. Additional studies implicated TGF- as the active EGFR ligand cleaved by TACE during wound repair. Reactive oxygen species scavengers, NADPH oxidase inhibitors, and importantly small interfering RNA of dual oxidase 1 inhibited LPS-induced wound repair. Inhibitors of protein kinase C isoforms and a TLR-4 neutralizing Ab also inhibited LPS-induced wound repair. Normal human bronchial epithelial cells responded similarly. Thus, LPS accelerates wound repair in airway epithelial cells via a novel TLR-4protein kinase C dual oxidase 1reactive oxygen speciesTACETGF-EGFR phosphorylation pathway.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
When bacteria are inhaled and deposit in the airways, the epithelium responds, initiating a dynamic interaction between host and pathogen (1, 2). Thus, the surface of the airway epithelium can be considered a battleground in which the host intercepts signals from pathogens and activates epithelial defenses to combat infection. Airway injury damages the protective barrier of the airway epithelium, assisting invasion by pathogens. The host innate immune response involves a complex signaling cascade that releases cytokines to activate inflammation involving the following: 1) the recruitment of neutrophils that kill bacteria, 2) mucin production and subsequent mucociliary clearance, and 3) repair of epithelial cell damage (3, 4).

Gram-negative bacteria, especially Pseudomonas aeruginosa, are important in the pathophysiology of several chronic airway diseases, including cystic fibrosis (5), bronchiectasis (6), and chronic obstructive pulmonary disease exacerbations (7). An important virulence factor for this bacterium is P. aeruginosa LPS, which has a receptor on the airway epithelial surface, TLR-4 (8, 9). TLR-4 is a member of a family of receptors that identify pathogen-associated molecular patterns to signal a variety of innate immune responses (10, 11). Damage to the airway epithelium occurs in various chronic airway diseases (12, 13), and repair of the injured epithelium has been shown to involve activation of the epidermal growth factor receptor (EGFR)³ (14, 15), which is located on the airway epithelial surface (16). P. aeruginosa and its virulence factors are known to be toxic and to damage the airway epithelium (17, 18, 19), inhibiting wound repair (20, 21, 22). However, because the epithelium is capable of responding to inhaled pathogens to produce innate immune signaling, we hypothesized that the airway epithelium responds to the presence of nontoxic levels of Gram-negative bacterial product Pseudomonas LPS by accelerating wound repair. We describe a novel surface pathway that stimulates wound repair. This signaling pathway includes TLR-4, protein kinase C (PKC) , dual oxidase 1 (Duox1), reactive oxygen species (ROS), TNF--converting enzyme (TACE), TGF-, and EGFR phosphorylation.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Materials

AG-1478, AG-1295, TNF- proteinase inhibitor-1 (TAPI-1), EGFR neutralizing Ab (Ab 3), epidermal growth factor (EGF) neutralizing Ab, TGF- neutralizing Ab (Ab 3), GM-6001, TGF-, apocynin, diphenyleneiodonium chloride (DPI), Gö6976, Gö6983, N^G-monoethyl-L-arginine (NMEA), and rottlerin were purchased from Calbiochem. Amphiregulin and heparin-binding EGF (HB-EGF) neutralizing Abs were purchased from Santa Cruz Biotechnology. DMSO, n-propyl gallete (nPG), P. aeruginosa LPS serotype 10, and allopurinol were obtained from Sigma-Aldrich. TLR-4 neutralizing mAb (HTA-125) and TLR-3 neutralizing mAb were purchased from eBioscience.

Cell culture

Cells from the human pulmonary mucoepidermoid carcinoma cell line, NCI-H292, were plated at 1.0 x 10⁵ cells/cm² in 24-well plates (BD Falcon). Cells were grown in RPMI 1640 medium (Cell Culture Facility, University of California, San Francisco) containing 10% FCS, penicillin (100 U/ml), streptomycin (100 µg/ml), and HEPES (25 mM) at 37°C in a humidified 5% CO₂ water-jacketed incubator. Because cell lines such as NCI-H292 cells show some variability in their response to stimuli and inhibitors at different passages (23), all experiments were performed in passages 80–90.

To confirm the results seen in NCI-H292 cells, limited experiments were also performed in normal human bronchial epithelial (NHBE) cells, which were purchased from Cambrex. Cells were passaged, seeded (in 24-well plates (BD Falcon) at 1.0 x 10⁵ cells/cm²), and grown to confluence. Cells were grown in bronchial epithelial growth medium (Cambrex) supplemented with defined growth factors contained in the Single-Quot kit (Cambrex) at 37°C in a humidified 5% CO₂ water-jacketed incubator.

Wound repair assay

NCI-H292 and NHBE cells were cultured in 24-well plates to confluence. A linear scratch wound was made with a 10-µl pipette tip in each well and washed with serum-free medium to remove cell debris, as described previously (14). The wounds were treated with LPS (10 µg/ml) with or without inhibitors, or with serum-free medium alone (control). Selected images were recorded continuously using an inverted microscope and digital video camera (Nikon TE2000-E) at 37°C and 5% CO₂. SimplePCI 5.1 software (Technical Instruments) converted individual images into videos. Images, at 1-h intervals, were converted to TIFF files (Adobe Photoshop 8.0) and analyzed with image analysis software (NIH ImageJ 1.33u). Wound area was measured at 2-h intervals for 12 h. Initial experiments established an orderly rate of repair, so subsequent experiments analyzed the initial wound area compared with the area at 12 h. Wound repair was expressed as a percentage of the initial wound area measured at the start of the experiment ((initial wound area – 12-h wound area)/initial wound area x 100 = % wound repair).

Cytotoxicity assay

Lactate dehydrogenase (LDH) activity was measured in the supernatants of all wound repair samples. LDH release was measured at 12 h, using a cytotoxicity detection kit (Roche), according to the manufacturer’s protocol. There were no differences in LDH between control and treated wounds (data not shown), except at high concentrations of LPS (see Results; Fig. 1). Results are represented as percentage of LDH released into the supernatant ((supernatant/supernatant + lysate) x 100 = % LDH release).

View larger version (17K): [in this window] [in a new window]   FIGURE 1. Concentration-dependent effects of LPS on wound repair. Wound repair was evaluated at 12 h with serum-free medium plus increasing concentrations of LPS (0–500 µg/ml: columns, y-axis, left). Percentage of LDH released into the supernatant was measured ((supernatant/supernatant + lysate) x 100 = % LDH release) (solid line, y-axis, right). Data are means ± SD (n = 3; #, p < 0.05 vs 300, 500 µg/ml; *, p < 0.01 vs 0, 100, 300, 500 µg/ml).

Release of soluble TGF- in the wound repair assay

NCI-H292 cells were cultured in 24-well plates, as described above. After reaching confluence, cells were serum starved for 24 h before wounding. In these studies, cells were pretreated with inhibitors for 30 min in addition to EGFR neutralizing Ab (4 µg/ml), which prevents soluble TGF- from binding to EGFR. To maximize the release of soluble EGFR ligands, multiple wounds were made in each well: a pipette tip was used to make five parallel linear scratch wounds, and then each well was rotated 90° and another five parallel linear scratch wounds were made. The wounds were washed to remove debris, and then an EGFR neutralizing Ab (4 µg/ml) and LPS (10 µg/ml), with or without inhibitors, were added to serum-free medium. After 2 h, cell supernatants were collected, and TGF- was measured with a TGF- ELISA kit (Oncogene Research Products), according to the manufacturer’s protocol. Total protein in cell lysates was measured using the bicinchoninic acid protein assay kit (Pierce Biotechnology), and results are represented as TGF- (pg)/total protein (µg) to normalize for possible differences in cell number.

TACE and Duox1 small interfering RNA (siRNA) preparation and transfection

Predesigned human TACE siRNAs (104029, 104030, and 104031) were purchased from Ambion. In preliminary studies, TACE siRNA 104029 (300 nM) inhibited LPS-induced wound repair significantly. Therefore, this siRNA was selected for subsequent studies. The 21-nt sequences for TACE (siRNA 104029) were GGUUUUAAAGGCUAUGGAAtt (sense) and UUCCAUAGCCUUUAAAACCtg (antisense). Predesigned human Duox1 siRNAs (24873 and 24969) were purchased from Ambion. In preliminary studies, Duox1 siRNA 24873 (100 nM) inhibited LPS-induced wound repair significantly. Therefore, this siRNA was selected for subsequent studies. The 21-nt sequences for Duox1 (siRNA 24873) were GGACCAU GUGUUGGUUGAAtt (sense) and UUCAACCAACACAUGGUCCtc (antisense). Silencer Negative Control 1 siRNA (Ambion) was used as a nonspecific siRNA. siRNA transfection into NCI-H292 cells was conducted using Lipofectamine 2000 (Invitrogen Life Technologies) when cells were 40–50% confluent. When cells reached confluence, linear wounds were made and wound repair was measured, as described above. To determine siRNA transfection efficiency, FAM-labeled GADPH siRNA (Ambion) was transfected, as described. At the time wounds would have been made, the number of FAM-positive cells was counted by fluorescence microscopy. Transfection efficiency was >60% ((FAM-positive cells/total cells) x 100 = % transfection efficiency). Specific silencing of TACE and of Duox1 was confirmed using RT-PCR.

RNA isolation, reverse transcription, and RT-PCR

Total RNA was isolated and reverse transcription was performed, as previously described (24, 25). Total RNA was isolated using RNAqueous-4PCR kit (Ambion), and 2 µg was primed with oligo(dT) and reverse transcribed using a RETROscript kit (Ambion) in a final volume of 20 µl (RT reaction), according to the manufacturer’s instructions. Two microliters of the reverse-transcriptase reaction was PCR amplified in a 50-µl reaction. The following primers were used: Duox1, 5'-GCCCTGTACAACCAGGACTT-3' (forward) and 5'-CGCACAAATTGTTCAAGGAC-3' (reverse); TACE, 5'-ACCTGAAGAGCTTGTTCATCGAG-3' (forward) and 5'-CCATGAAGTGTTCCGATAGATGTC-3' (reverse). As internal controls, primers for Rig/S15 rRNA, a housekeeping gene that is constitutively expressed, were used. They were 5'-TTCCGCAAGTTCACCTACC-3' (forward) and 5'-CGGGCCGGCCATGCTTTACG-3' (reverse). The PCR mixture was denatured at 94°C for 5 min, followed by 38 cycles at 94°C for 30 s, 57°C for 45 s, and 72°C for 45 s. After PCR, 10-µl aliquots were subjected to 1.5% agarose gel electrophoresis and stained with ethidium bromide.

Immunocytochemical staining

Cells grown on four-chamber slides (Nunc) were serum starved for 24 h before experiments to maintain low basal levels of phosphorylation. For inhibition studies, cells were pretreated with a PKC inhibitor (Gö6976; 70 nM; Calbiochem) for 30 min before making a scratch wound. The wounds were washed to remove cellular debris, and LPS (10 µg/ml), Gö6976, or serum-free medium (control) was added. After 30 min, wounds were washed, fixed, and stained, as described previously (26), using rabbit mAbs to PKC isoforms (1/100; Cell Signaling Technology). Consecutive cells at the wound margin were analyzed at x40, positive staining cells were counted, and the percentage of PKC -positive cells was calculated (27).

Statistical analysis

Data are presented as means ± SD (n = 3). ANOVA was used to determine statistically significant differences (p < 0.05).

	Results

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Effect of LPS concentration on wound repair

P. aeruginosa products such as LPS are known to cause pulmonary epithelial damage (19). We hypothesized that the outcome of LPS-induced repair in epithelial wounding depends on the balance between epithelial protective responses and potential epithelial damage by the bacterial products. We found that a low concentration of LPS (10 µg/ml) accelerated wound repair (Fig. 1), but higher LPS concentrations resulted in decreased wound repair; at 500 µg/ml LPS, wound repair was inhibited completely (Fig. 1). At higher concentrations of LPS, the decrease in wound repair was associated with increasing LDH release (Fig. 1), an indication of epithelial cell damage.

Addition of EGFR ligand (TGF-) or Pseudomonas bacterial product (LPS) accelerates wound repair via EGFR phosphorylation

In the control state, wound area decreased in an orderly fashion over 12 h; the EGFR ligand, TGF- (10 ng/ml), accelerated wound repair (Fig. 2A). The addition of a selective EGFR tyrosine kinase inhibitor, AG 1478 (10 µM), inhibited wound repair both in the control state and with the addition of TGF- (Fig. 2A). From these results, we conclude that EGFR activation modulates wound repair in NCI-H292 cells.

View larger version (13K): [in this window] [in a new window]   FIGURE 2. Effects of TGF- and LPS on wound repair. Confluent cultures of NCI-H292 cells were wounded, and wound closure was recorded continuously by time-lapse videomicroscopy. A, Wound repair was measured over 12 h with serum-free medium alone (control, •) or with the addition of TGF-, an EGFR ligand (10 ng/ml, ). Control- and TGF--treated wounds were treated with an EGFR phosphorylation inhibitor, AG 1478 (10 µM) (control + AG 1478, ; TGF- + AG1478, ). Results are expressed as percentage of wound repair. Data are means ± SD (n = 3; *, p < 0.05 vs control and TGF- + AG 1478; #, p < 0.05 vs control + AG 1478). B, Wound repair was measured over 12 h with serum-free medium alone (control, •) or with the addition of LPS (10 µg/ml, ). Control- and LPS-treated wounds were treated with AG 1478 (10 µM) (control + AG 1478, ; LPS + AG 1478, ). Results are expressed as percentage of wound repair. Data are means ± SD (n = 3; *, p < 0.05 vs control and LPS + AG 1478; #, p < 0.05 vs control + AG 1478).

Ligand-dependent EGFR activation and the EGFR ligand TGF- mediate LPS-induced wound repair

Treatment of wounds with an EGFR neutralizing Ab (4 µg/ml), which blocks ligand binding sites on EGFR and inhibits subsequent EGFR phosphorylation, prevented LPS-accelerated wound repair (Fig. 3A), implicating ligand-dependent EGFR phosphorylation in the response to LPS. Treatment with a TGF- neutralizing Ab (4 µg/ml) (Fig. 3A) also inhibited LPS-induced wound repair. This inhibition was not seen with the addition of neutralizing Abs (4 µg/ml) to EGF, amphiregulin, or HB-EGF (data not shown). In addition, measurement of TGF- released into cell supernatant showed a significant increase in the presence of LPS compared with control (59.3 ± 9.5 vs 31.5 ± 0.8 pg/µg total protein; p < 0.05; n = 3). These results implicate the EGFR ligand, TGF-, in LPS-accelerated wound repair in NCI-H292 cells.

View larger version (22K): [in this window] [in a new window]   FIGURE 3. LPS-induced wound repair involves ligand-dependent EGFR activation, the EGFR ligand TGF-, and the metalloprotease TACE. A, Wound repair was analyzed at 12 h with serum-free medium (control, left column) or with the addition of LPS (10 µg/ml, second column). A neutralizing EGFR Ab (EGFR Ab, 4 µg/ml, third column) or a neutralizing Ab to TGF- (TGF- Ab, 4 µg/ml, fourth column) was added to LPS-treated wounds. Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + EGFR Ab; +, p < 0.05 vs LPS + TGF- Ab). B, A general metalloprotease inhibitor, GM 6001 (10 µM, third column), or a more selective TACE inhibitor, TAPI-1 (TAPI, 10 µM, fourth column), was added to LPS-treated wounds. Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + GM6001; +, p < 0.05 vs LPS + TAPI). C, NCI-H292 cells were transfected with or without TACE siRNA and cultured for 72 h, and then analyzed for TACE mRNA expression by RT-PCR. Cells were transfected with Lipofectamine (Invitrogen Life Technologies) alone (vehicle), TACE siRNA (300 µM), nonspecific siRNA (300 µM), or no treatment (control). Rig/S15 was used as an internal marker. D, NCI-H292 cells were transfected with TACE siRNA and wounded. Wound repair was analyzed at 12 h with serum-free medium (control, left three columns) plus Lipofectamine (vehicle, 1.5 µl/500 µl total volume) and TACE siRNA (300 µM), or a nonspecific siRNA sequence (300 µM). These results were compared with wounds treated with LPS (10 µg/ml, right three columns) plus Lipofectamine (vehicle, 1.5 µl/500 µl total volume) and TACE siRNA (300 µM), or a nonspecific siRNA sequence (300 µM). Data are means ± SD (n = 3; #, p < 0.05 vs TACE; *, p < 0.01 vs TACE).

The metalloprotease TACE is known to cleave and release the EGFR proligand TGF- from the epithelial surface in airway epithelial cells (25), allowing the cleaved ligand to bind to and phosphorylate EGFR. In this study, we found that a general metalloprotease inhibitor, GM6001 (10 µM), and a more selective TACE inhibitor, TAPI-1 (10 µM), prevented LPS-accelerated wound repair (Fig. 3B). In addition, release of TGF- into the cell supernatant was prevented by pretreatment with TAPI-1 (10 µM) compared with LPS alone (18.5 ± 0.6 vs 59.3 ± 9.5 pg/µg total protein; p < 0.05; n = 3). These results implicate a metalloprotease, perhaps TACE, and the cleavage and release of the EGFR ligand TGF- in wound repair induced by LPS.

siRNA knockdown of TACE prevents LPS-induced wound repair

Because TACE cleaves pro-TGF- (28), we examined whether TACE is involved in LPS-induced wound repair. We used siRNA to knockdown TACE expression in NCI-H292 cells. In the control state, TACE siRNA (300 µM) decreased TACE mRNA expression (Fig. 3C) and suppressed wound repair (Fig. 3D). LPS-accelerated wound repair was also markedly decreased (Fig. 3D). A nonspecific control siRNA (300 µM) was without effect in both the control and LPS-treated wounds (Fig. 3D). These results implicate TACE in LPS-accelerated wound repair.

ROS mediate LPS-induced wound repair

ROS are reported to activate TACE (24). In this study, we found that the ROS scavengers, nPG (100 µM) and DMSO (1%), prevented LPS-induced wound repair (Fig. 4). TGF- released into cell supernatant was inhibited by pretreatment with nPG (100 µM) compared with LPS alone (31.7 ± 14.0 vs 59.3 ± 9.5 pg/µg total protein; p < 0.05; n = 3). These results implicate ROS in response to LPS.

View larger version (16K): [in this window] [in a new window]   FIGURE 4. Effect of ROS scavengers on LPS-induced wound repair. Wound repair was measured at 12 h with serum-free medium (control, left column) or with the addition of LPS (10 µg/ml, second column). ROS scavengers nPG (100 µM, third column) or DMSO (1%, fourth column) were added to the LPS-treated wounds. Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + nPG; +, p < 0.05 vs LPS + DMSO).

Nox are known to generate ROS in airway epithelial cells by a core component homolog Duox1 (29, 30). In this study, we found that general Nox inhibitors (DPI (1.0 µM) or apocynin (1.0 mM)) prevented LPS-induced wound repair (Fig. 5A). To exclude the involvement of other oxidases, we investigated the effect of inhibitors of xanthine oxidases (allopurinol (100 µM), NO synthase, and NMEA (100 µM)). These inhibitors had no significant effect on LPS-induced wound repair (Fig. 5A). These results implicate Nox in LPS-induced wound repair.

View larger version (23K): [in this window] [in a new window]   FIGURE 5. LPS-induced wound repair involves Nox and Duox1. A, Wound repair was analyzed at 12 h with serum-free medium (control, left column) or with the addition of LPS (10 µg/ml, second column). A general Nox inhibitor DPI (1.0 µM, third column) or apocynin (APO, 1.0 mM, fourth column) was added to LPS-treated wounds. A NO inhibitor, NMEA (100 µM, fifth column), or a xanthine oxidase inhibitor, allopurinol (ALP 100 µM, sixth column), was added to LPS-treated wounds. Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + DPI; +, p < 0.05 vs LPS + APO). B, NCI-H292 cells were transfected with or without Duox1 siRNA and cultured for 72 h, and then analyzed for Duox1 mRNA expression by RT-PCR. Cells were transfected with Lipofectamine (Invitrogen Life Technologies) alone (vehicle), Duox1 siRNA (100 µM), nonspecific siRNA (100 µM), or no treatment (control). Rig/S15 was used as an internal marker. C, NCI-H292 cells were transfected with Duox1 siRNA and wounded. Wound repair was analyzed at 12 h with serum-free medium (control, left three columns) plus Lipofectamine (vehicle, 1.5 µl/500 µl total volume), Duox1 siRNA (100 µM), or a nonspecific siRNA sequence (100 µM). These results were compared with wounds treated with LPS (10 µg/ml, right three columns) plus Lipofectamine (vehicle, 1.5 µl/500 µl total volume), Duox1 siRNA (Duox1, 100 µM), or a nonspecific siRNA sequence (100 µM). Data are means ± SD (n = 3; #, p < 0.01 vs Duox1; *, p < 0.01 vs Duox1).

Recently, Duox1, a gp91^phox homolog in airway epithelial cells, has been shown to activate TACE via ROS production (24). We studied the effects of siRNA knockdown of Duox1 expression in NCI-H292 cells. In the control state, Duox1 siRNA (100 µM) inhibited Duox1 mRNA expression (Fig. 5B) and noticeably inhibited wound repair (Fig. 5C). LPS-induced wound repair was also markedly inhibited by Duox1 siRNA (Fig. 5C). A nonspecific control siRNA (100 µM) was without effect in both control and LPS-treated wounds (Fig. 5C). These results implicate Duox1 in control- and in LPS-induced wound repair.

Calcium-dependent PKC isoforms mediate LPS-induced wound repair

PKC isoforms have been described to activate Nox (31). The PKC isoforms can be divided into two general categories: Ca²⁺ dependent (, , ) or Ca²⁺ independent (, , , , ). LPS has been shown to stimulate activation of both calcium-dependent and calcium-independent isoforms, including PKC , , , and (32, 33, 34). In this study, we found that a general PKC inhibitor Gö6983 (70 nM) prevented LPS-induced wound repair (Fig. 6A). A PKC (Ca²⁺-dependent)-selective inhibitor, Gö6976 (70 nM), also inhibited LPS-induced wound repair, whereas a PKC (Ca²⁺- independent)-selective inhibitor, rottlerin (3 µM), had no significant effect (Fig. 6A). PKC phosphorylation at the wound margin was evaluated by immunocytochemistry. The addition of LPS (10 µg/ml) increased PKC phosphorylation at the wound margin compared with control (Fig. 6, B and C), an effect that was decreased in wounds pretreated with PKC inhibitor, Gö6976 (Fig. 6, B and C). These results implicate Ca²⁺- dependent PKC in LPS-induced wound repair.

View larger version (40K): [in this window] [in a new window]   FIGURE 6. LPS-induced wound repair involves Ca2+-dependent PKC . A, Wound repair was measured at 12 h with serum-free medium alone (control; left column) or with the addition of LPS (10 µg/ml; second column). A general PKC inhibitor, Gö6983 (PKC gen, 70 nM, third column), or a more selective PKC (Ca2+-dependent) inhibitor, Gö6976 (PKC , 70 nM, fourth column), was added to the LPS-treated wounds. These results are compared with a PKC (Ca2+-independent)-selective inhibitor rottlerin (PKC , 3 µM, fifth column). Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + Gö6983 (PKC gen); +, p < 0.05 vs LPS + Gö6976 (PKC )). B, Photomicrographs of PKC phosphorylation at the wound edge. Cells were stained for phospho-PKC in wounds with serum-free medium alone (control), with the addition of LPS (10 µg/ml), or with LPS (10 µg/ml) plus pretreatment with PKC inhibitor, Gö6976 (PKC Inhib, 70 nM). Photomicrographs are shown at x20 magnification and are representative of three separate experiments. Bar, 50 µm. C, Cells staining positive for phospho-PKC at the wound margin were counted with serum-free medium (control; left column), the addition of LPS (10 µg/ml; middle column), or pretreatment with PKC inhibitor, Gö6976 (PKC , 70 nM, right column), and percentage of PKC -positive cells was calculated. Data are means ± SD (n = 3 separate experiments; #, p < 0.01 vs control; *, p < 0.01 vs LPS + Gö6976 (PKC )).

To confirm the results of studies with NCI-H292 cells, selected experiments targeting critical steps in LPS-induced wound repair were also performed with NHBE cells. The addition of LPS (10 µg/ml) to NHBE cells accelerated wound repair compared with control (Fig. 7). This effect was inhibited by the addition of a selective EGFR tyrosine kinase inhibitor, AG 1478 (10 µM) (Fig. 7). A metalloprotease inhibitor that shows some selectivity for TACE, TAPI-1 (10 µM), prevented LPS-accelerated wound repair in NHBE cells (Fig. 7). A ROS scavenger, nPG (100 µM), inhibited LPS-induced wound repair (Fig. 7), and the addition of a general Nox inhibitor apocynin (1.0 mM) prevented LPS-induced wound repair in NHBE cells (Fig. 7). siRNA knockdown of TACE and Duox1 was not possible in NHBE cells. Finally, the addition of a PKC (Ca²⁺-dependent)-selective inhibitor, Gö6976 (70 nM), also inhibited LPS-induced wound repair. These results confirm the studies in NCI-H292 cells.

View larger version (14K): [in this window] [in a new window]   FIGURE 7. LPS-induced wound repair in NHBE cells. Wound repair in NHBE cells was measured at 12 h with serum-free medium (control, first column) or with the addition of LPS (10 µg/ml, second column), and selected inhibitors were added to confirm results seen in NCI-H292 cells. An EGFR tyrosine kinase phosphorylation inhibitor, AG 1478 (10 µM, third column), a metalloprotease inhibitor with some selectivity for TACE, TAPI-1 (TAPI, 10 µM, fourth column), a ROS scavenger nPG (100 µM, fifth column), a general Nox inhibitor apocynin (APO, 1.0 mM, sixth column), or a selective PKC (Ca2+-dependent) inhibitor, Gö6976 (PKC , 70 nM, seventh column), was added to LPS-treated wounds. Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + each inhibitor).

LPS is a ligand for TLR-4 (8, 9). A neutralizing Ab to TLR-4 (0.1 µg/ml) prevented LPS-induced acceleration of wound repair, but a TLR-3 neutralizing Ab (0.1 µg/ml) was without effect (Fig. 8). These results suggest that LPS binding to TLR-4 is involved in LPS-accelerated wound repair.

View larger version (18K): [in this window] [in a new window]   FIGURE 8. The role of TLR-4 in LPS-induced wound repair. Wound repair was evaluated at 12 h with serum-free medium (control, first column) or with the addition of LPS (10 µg/ml, second column). Neutralizing Abs to TLR-4 (0.1 µg/ml, third column) or TLR-3 (0.1 µg/ml, fourth column) were added to LPS-treated wounds. Data are means ± SD (n = 3; *, p < 0.05 vs control; #, p < 0.05 vs LPS + TLR-4 Ab).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

First, we showed that the effects of LPS are concentration dependent. Low concentrations of LPS increased wound repair, whereas higher concentrations decreased wound repair and were toxic to the airway epithelium. Because EGFR activation is known to regulate wound repair and because LPS, a secreted product of P. aeruginosa, causes EGFR activation (25), we investigated the role of EGFR phosphorylation in LPS-induced wound repair. Blockade of EGFR tyrosine kinase phosphorylation inhibited LPS-induced wound repair, implicating EGFR activation in the wound repair process. A family of growth factors (i.e., EGF, TGF-, HB-EGF, and amphiregulin) activates the EGFR. In alveolar (36), airway (15), corneal (37), keratinocyte (38), and intestinal (39) cell studies, the addition of growth factors activates EGFR and accelerates wound repair. In this study, we found that an EGFR neutralizing Ab, which prevents EGFR ligands from binding to the receptor, inhibits LPS-induced wound repair, implicating ligand-dependent EGFR activation in LPS-induced wound repair. Therefore, we examined the EGFR ligand involved in this airway epithelial response to LPS, using neutralizing Abs to various EGFR ligands to prevent their binding to EGFR. The addition of a TGF- neutralizing Ab inhibited LPS-induced wound repair, whereas neutralizing Abs to EGF, HB-EGF, and amphiregulin were without effect, suggesting that LPS induced the cleavage and release of TGF-, allowing it to bind to and activate EGFR. Furthermore, we showed that LPS caused the release of TGF- into the cell supernatant, confirming that TGF- release occurred in response to LPS. TGF- release has been measured in an intestinal wound model (40). In corneal (41, 42) and keratinocyte (43, 44) wound models, HB-EGF was implicated, suggesting that different EGFR ligands are involved in repair of various epithelia.

Next, we examined the mechanisms underlying LPS-induced TGF- release. Metalloproteases are known to cleave EGFR proligands and to release soluble ligands, making them available for binding to the EGFR (45). We hypothesized that during LPS-stimulated wound repair, a metalloprotease on the surface of epithelial cells releases soluble TGF-, allowing it to bind to and activate EGFR. Incubation of the wounds with a general metalloprotease inhibitor (GM 6001) prevented LPS-induced wound repair, implicating a metalloprotease in this process. A similar effect was seen using this general metalloprotease inhibitor in corneal (41, 42) and keratinocyte (46) wounds. TACE, a disintegrin and metalloprotease-17 family member present on the surface of airway epithelial cells, is known to cleave pro-TGF- and release soluble TGF- (28, 47). Addition of TAPI-1, a somewhat selective inhibitor of TACE, also prevented LPS-induced wound repair. This inhibitor was used in a model of intestinal wound repair (40). However, because TAPI-1 is not completely specific for TACE, we also examined the effect of siRNA knockdown of TACE on LPS-induced wound repair. siRNA is an effective means of silencing gene expression and protein production (48, 49). TACE siRNA prevented LPS-induced wound repair, implicating TACE as the metalloprotease involved in EGFR proligand cleavage.

Because ROS are known to activate TACE in the airway epithelium (24), we examined the role of ROS scavengers in wound repair. We showed that ROS scavengers inhibit LPS-induced wound repair. Next, we examined the mechanism of ROS production in this signaling cascade. Nox generate ROS production. The core component of Nox is the catalytic subunit glycoprotein p91^phox, and several homologs have been identified in various cell types (50, 51). Recently, TLR-4 activation was shown to generate ROS (52), and Park et al. (53) reported that TLR-4 has a direct interaction with Nox 4, one of the gp91^phox homologs. This interaction is essential for LPS-induced ROS production and activation of NF-B. In mice given P. aeruginosa, ROS production and NF-B activation required p47^phox, a cytosolic component of Nox (54). Recently, a homolog of the gp91^phox, Duox1, was identified in human airway epithelial cells and was found to generate ROS (30). In this study, we showed that selective inhibitors of Nox prevent LPS-induced wound repair. This effect was not seen with xanthine oxidase inhibitors nor with NO synthase inhibitors. Furthermore, because Duox1 siRNA decreased LPS-induced wound repair markedly, we conclude that Duox1 is involved in the LPS-induced generation of ROS.

To determine the mechanism of Duox1 activation, we examined the role of PKC. PKC isoforms are generally grouped as follows: 1) classical or calcium dependent (, , ), and 2) calcium independent (, ). In this study, we showed that selective inhibition of the calcium-dependent PKC , but not the calcium-independent PKC isoforms, prevents LPS-induced repair. In addition, LPS increased PKC phosphorylation at the wound margin, further implicating PKC in this signaling cascade. Because PKC signaling of mucin production is upstream of Duox1 (24), our results suggest that PKC activates Duox1 in LPS-induced airway epithelial wound repair. Finally, to determine whether TLR-4 is required for LPS binding, we added a TLR-4 neutralizing Ab to the wounded epithelium. Addition of this Ab inhibited LPS-induced wound repair. Thus, binding of LPS to its receptor initiates an epithelial cell surface signaling cascade that activates the EGFR and stimulates wound repair.

In summary, present studies show that LPS, a bacterial product of Gram-negative bacteria, causes accelerated wound repair in airway epithelial cells via a TLR-4PKC DUOX1ROSTACETGF-EGFR phosphorylation pathway (Fig. 9). In addition, we showed that the effects of LPS are concentration dependent: low concentrations of LPS increased wound repair, whereas higher concentrations decreased wound repair and were toxic to the airway epithelium. The response to low concentrations of LPS suggests that the airway epithelium provides an important function by intercepting signals from pathogens and activating host defenses. In contrast, higher concentrations of LPS overcome this response and cause cytotoxicity that may initiate epithelial damage and facilitate invasion. In addition to wound repair, important host defenses include recruitment of neutrophils to kill pathogens and production of mucins to assist in their clearance. We suggest that high concentrations of pathogens may also overwhelm these innate immune defenses to cause pathology or to exacerbate chronic airway diseases.

View larger version (16K): [in this window] [in a new window]   FIGURE 9. Diagrammatic scheme of LPS-induced wound repair. LPS binds to its receptor, TLR-4, to activate PKC isoforms PKC and PKC. Duox1 is then activated, generating ROS (represented by ). ROS activate the latent form of TACE, which has an inhibitory prodomain (represented by the curved black line) covering its active domain (represented by scissors), removing the prodomain and exposing the active domain to cleave pro-TGF-. Soluble TGF- is released, which binds to and activates EGFR, initiating signaling for wound repair.

	Acknowledgments

 
We thank Drs. Michael Matthay, Joanne Engel, and Sasha Shafikhani (all at the University of California, San Francisco) for their generous advice regarding wound repair assays and access to videomicroscopy equipment, and Dr. Julien Hoffman (University of California, San Francisco) for assistance with statistical analysis.

	Disclosures

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
The authors have no financial conflict of interest.

	Footnotes

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ This work was supported by Cardiovascular Research Institute funding.

² Address correspondence and reprint requests to Dr. Jay A. Nadel, University of California, San Francisco, 505 Parnassus Avenue, Room S-1183, San Francisco, CA 94143-0130. E-mail address: jay.nadel{at}ucsf.edu

³ Abbreviations used in this paper: EGFR, epidermal growth factor receptor; DPI, diphenyleneiodonium chloride; Duox1, dual oxidase 1; EGF, epidermal growth factor; HB-EGF, heparin-binding EGF; LDH, lactate dehydrogenase; NHBE, normal human bronchial epithelial; NMEA, N^G-monoethyl-L-arginine; Nox, NADPH oxidase; nPG, n-propyl gallete; PKC, protein kinase C; ROS, reactive oxygen species; siRNA, small interfering RNA; TACE, TNF--converting enzyme; TAPI-1, TNF- proteinase inhibitor-1.

Received for publication June 23, 2006. Accepted for publication September 28, 2006.

	References

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 

1. Kunzelmann, K., B. McMorran. 2004. First encounter: how pathogens compromise epithelial transport. Physiology 19: 240-244. [Abstract/Free Full Text]
2. Kazmierczak, B. I., K. Mostov, J. N. Engel. 2001. Interaction of bacterial pathogens with polarized epithelium. Annu. Rev. Microbiol. 55: 407-435. [Medline]
3. Knowles, M. R., R. C. Boucher. 2002. Mucus clearance as a primary innate defense mechanism for mammalian airways. J. Clin. Invest. 109: 571-577. [Medline]
4. Whitsett, J. A.. 2002. Intrinsic and innate defenses in the lung: intersection of pathways regulating lung morphogenesis, host defense, and repair. J. Clin. Invest. 109: 565-569. [Medline]
5. Gibson, R. L., J. L. Burns, B. W. Ramsey. 2003. Pathophysiology and management of pulmonary infections in cystic fibrosis. Am. J. Respir. Crit. Care Med. 168: 918-951. [Abstract/Free Full Text]
6. Barker, A. F.. 2002. Bronchiectasis. N. Engl. J. Med. 346: 1383-1384. [Free Full Text]
7. Sethi, S., N. Evans, B. J. Grant, T. F. Murphy. 2002. New strains of bacteria and exacerbations of chronic obstructive pulmonary disease. N. Engl. J. Med. 347: 465-471. [Abstract/Free Full Text]
8. Hoshino, K., O. Takeuchi, T. Kawai, H. Sanjo, T. Ogawa, Y. Takeda, K. Takeda, S. Akira. 1999. Cutting edge: Toll-like receptor 4 (TLR4)-deficient mice are hyporesponsive to lipopolysaccharide: evidence for TLR4 as the Lps gene product. J. Immunol. 162: 3749-3752. [Abstract/Free Full Text]
9. Medzhitov, R., P. Preston-Hurlburt, C. A. Janeway, Jr. 1997. A human homologue of the Drosophila Toll protein signals activation of adaptive immunity. Nature 388: 394-397. [Medline]
10. Akira, S., K. Takeda, T. Kaisho. 2001. Toll-like receptors: critical proteins linking innate and acquired immunity. Nat. Immunol. 2: 675-680. [Medline]
11. Akira, S., S. Uematsu, O. Takeuchi. 2006. Pathogen recognition and innate immunity. Cell 124: 783-801. [Medline]
12. Baltimore, R. S., C. D. Christie, G. J. Smith. 1989. Immunohistopathologic localization of Pseudomonas aeruginosa in lungs from patients with cystic fibrosis: implications for the pathogenesis of progressive lung deterioration. Am. Rev. Respir. Dis. 140: 1650-1661. [Medline]
13. Jeffery, P. K.. 2001. Remodeling in asthma and chronic obstructive lung disease. Am. J. Respir. Crit. Care Med. 164: S28-S38. [Abstract/Free Full Text]
14. Matthay, M. A., J. P. Thiery, F. Lafont, F. Stampfer, B. Boyer. 1993. Transient effect of epidermal growth factor on the motility of an immortalized mammary epithelial cell line. J. Cell Sci. 106: 869-878. [Abstract]
15. Puddicombe, S. M., R. Polosa, A. Richter, M. T. Krishna, P. H. Howarth, S. T. Holgate, D. E. Davies. 2000. Involvement of the epidermal growth factor receptor in epithelial repair in asthma. FASEB J. 14: 1362-1374. [Abstract/Free Full Text]
16. Takeyama, K., K. Dabbagh, H. M. Lee, C. Agusti, J. A. Lausier, I. F. Ueki, K. M. Grattan, J. A. Nadel. 1999. Epidermal growth factor system regulates mucin production in airways. Proc. Natl. Acad. Sci. USA 96: 3081-3086. [Abstract/Free Full Text]
17. Kurahashi, K., O. Kajikawa, T. Sawa, M. Ohara, M. A. Gropper, D. W. Frank, T. R. Martin, J. P. Wiener-Kronish. 1999. Pathogenesis of septic shock in Pseudomonas aeruginosa pneumonia. J. Clin. Invest. 104: 743-750. [Medline]
18. Wilson, R., R. B. Dowling, A. D. Jackson. 1996. The effects of bacterial products on airway cells and their function. Am. J. Respir. Crit. Care Med. 154: S197-S201. [Medline]
19. Sadikot, R. T., T. S. Blackwell, J. W. Christman, A. S. Prince. 2005. Pathogen-host interactions in Pseudomonas aeruginosa pneumonia. Am. J. Respir. Crit. Care Med. 171: 1209-1223. [Abstract/Free Full Text]
20. De Bentzmann, S., M. Polette, J. M. Zahm, J. Hinnrasky, C. Kileztky, O. Bajolet, J. M. Klossek, A. Filloux, A. Lazdunski, E. Puchelle. 2000. Pseudomonas aeruginosa virulence factors delay airway epithelial wound repair by altering the actin cytoskeleton and inducing overactivation of epithelial matrix metalloproteinase-2. Lab. Invest. 80: 209-219. [Medline]
21. Garrity-Ryan, L., S. Shafikhani, P. Balachandran, L. Nguyen, J. Oza, T. Jakobsen, J. Sargent, X. Fang, S. Cordwell, M. A. Matthay, J. N. Engel. 2004. The ADP ribosyltransferase domain of Pseudomonas aeruginosa ExoT contributes to its biological activities. Infect. Immun. 72: 546-558. [Abstract/Free Full Text]
22. Geiser, T. K., B. I. Kazmierczak, L. K. Garrity-Ryan, M. A. Matthay, J. N. Engel. 2001. Pseudomonas aeruginosa ExoT inhibits in vitro lung epithelial wound repair. Cell. Microbiol. 3: 223-236. [Medline]
23. Zhang, Y., A. Wolf-Yadlin, P. L. Ross, D. J. Pappin, J. Rush, D. A. Lauffenburger, F. M. White. 2005. Time-resolved mass spectrometry of tyrosine phosphorylation sites in the epidermal growth factor receptor signaling network reveals dynamic modules. Mol. Cell. Proteomics 4: 1240-1250. [Abstract/Free Full Text]
24. Shao, M. X., J. A. Nadel. 2005. Dual oxidase 1-dependent MUC5AC mucin expression in cultured human airway epithelial cells. Proc. Natl. Acad. Sci. USA 102: 767-772. [Abstract/Free Full Text]
25. Shao, M. X., I. F. Ueki, J. A. Nadel. 2003. Tumor necrosis factor -converting enzyme mediates MUC5AC mucin expression in cultured human airway epithelial cells. Proc. Natl. Acad. Sci. USA 100: 11618-11623. [Abstract/Free Full Text]
26. Takeyama, K., K. Dabbagh, J. Jeong Shim, T. Dao-Pick, I. F. Ueki, J. A. Nadel. 2000. Oxidative stress causes mucin synthesis via transactivation of epidermal growth factor receptor: role of neutrophils. J. Immunol. 164: 1546-1552. [Abstract/Free Full Text]
27. Takeyama, K., B. Jung, J. J. Shim, P. R. Burgel, T. Dao-Pick, I. F. Ueki, U. Protin, P. Kroschel, J. A. Nadel. 2001. Activation of epidermal growth factor receptors is responsible for mucin synthesis induced by cigarette smoke. Am. J. Physiol. 280: L165-L172.
28. Peschon, J. J., J. L. Slack, P. Reddy, K. L. Stocking, S. W. Sunnarborg, D. C. Lee, W. E. Russell, B. J. Castner, R. S. Johnson, J. N. Fitzner, et al 1998. An essential role for ectodomain shedding in mammalian development. Science 282: 1281-1284. [Abstract/Free Full Text]
29. De Deken, X., D. Wang, M. C. Many, S. Costagliola, F. Libert, G. Vassart, J. E. Dumont, F. Miot. 2000. Cloning of two human thyroid cDNAs encoding new members of the NADPH oxidase family. J. Biol. Chem. 275: 23227-23233. [Abstract/Free Full Text]
30. Geiszt, M., J. Witta, J. Baffi, K. Lekstrom, T. L. Leto. 2003. Dual oxidases represent novel hydrogen peroxide sources supporting mucosal surface host defense. FASEB J. 17: 1502-1504. [Abstract/Free Full Text]
31. Suzuki, Y., R. I. Lehrer. 1980. NAD(P)H oxidase activity in human neutrophils stimulated by phorbol myristate acetate. J. Clin. Invest. 66: 1409-1418. [Medline]
32. Aksoy, E., M. Goldman, F. Willems. 2004. Protein kinase C: a new target to control inflammation and immune-mediated disorders. Int. J. Biochem. Cell Biol. 36: 183-188. [Medline]
33. Asehnoune, K., D. Strassheim, S. Mitra, J. Yeol Kim, E. Abraham. 2005. Involvement of PKC in TLR4 and TLR2 dependent activation of NF-B. Cell. Signal. 17: 385-394. [Medline]
34. Kim, D. C., S. H. Kim, M. W. Jeong, N. I. Baek, K. T. Kim. 2005. Effect of rottlerin, a PKC- inhibitor, on TLR-4-dependent activation of murine microglia. Biochem. Biophys. Res. Commun. 337: 110-115. [Medline]
35. Zahm, J. M., M. Chevillard, E. Puchelle. 1991. Wound repair of human surface respiratory epithelium. Am. J. Respir. Cell Mol. Biol. 5: 242-248. [Medline]
36. Kheradmand, F., H. G. Folkesson, L. Shum, R. Derynk, R. Pytela, M. A. Matthay. 1994. Transforming growth factor- enhances alveolar epithelial cell repair in a new in vitro model. Am. J. Physiol. 267: L728-L738. [Medline]
37. Song, Q. H., R. P. Singh, V. Trinkaus-Randall. 2001. Injury and EGF mediate the expression of ₆₄ integrin subunits in corneal epithelium. J. Cell. Biochem. 80: 397-414. [Medline]
38. Hebda, P. A.. 1988. Stimulatory effects of transforming growth factor- and epidermal growth factor on epidermal cell outgrowth from porcine skin explant cultures. J. Invest. Dermatol. 91: 440-445. [Medline]
39. Frey, M. R., A. Golovin, D. B. Polk. 2004. Epidermal growth factor-stimulated intestinal epithelial cell migration requires Src family kinase-dependent p38 MAPK signaling. J. Biol. Chem. 279: 44513-44521. [Abstract/Free Full Text]
40. Myhre, G. M., M. Toruner, S. Abraham, L. J. Egan. 2004. Metalloprotease disintegrin-mediated ectodomain shedding of EGFR ligands promotes intestinal epithelial restitution. Am. J. Physiol. 287: G1213-G1219.
41. Block, E. R., A. R. Matela, N. SundarRaj, E. R. Iszkula, J. K. Klarlund. 2004. Wounding induces motility in sheets of corneal epithelial cells through loss of spatial constraints: role of heparin-binding epidermal growth factor-like growth factor signaling. J. Biol. Chem. 279: 24307-24312. [Abstract/Free Full Text]
42. Xu, K. P., Y. Ding, J. Ling, Z. Dong, F. S. Yu. 2004. Wound-induced HB-EGF ectodomain shedding and EGFR activation in corneal epithelial cells. Invest. Ophthalmol. Visual Sci. 45: 813-820. [Abstract/Free Full Text]
43. Shirakata, Y., R. Kimura, D. Nanba, R. Iwamoto, S. Tokumaru, C. Morimoto, K. Yokota, M. Nakamura, K. Sayama, E. Mekada, et al 2005. Heparin-binding EGF-like growth factor accelerates keratinocyte migration and skin wound healing. J. Cell Sci. 118: 2363-2370. [Abstract/Free Full Text]
44. Tokumaru, S., S. Higashiyama, T. Endo, T. Nakagawa, J. I. Miyagawa, K. Yamamori, Y. Hanakawa, H. Ohmoto, K. Yoshino, Y. Shirakata, et al 2000. Ectodomain shedding of epidermal growth factor receptor ligands is required for keratinocyte migration in cutaneous wound healing. J. Cell Biol. 151: 209-220. [Abstract/Free Full Text]
45. Sunnarborg, S. W., C. L. Hinkle, M. Stevenson, W. E. Russell, C. S. Raska, J. J. Peschon, B. J. Castner, M. J. Gerhart, R. J. Paxton, R. A. Black, D. C. Lee. 2002. Tumor necrosis factor- converting enzyme (TACE) regulates epidermal growth factor receptor ligand availability. J. Biol. Chem. 277: 12838-12845. [Abstract/Free Full Text]
46. Mirastschijski, U., C. J. Haaksma, J. J. Tomasek, M. S. Agren. 2004. Matrix metalloproteinase inhibitor GM 6001 attenuates keratinocyte migration, contraction and myofibroblast formation in skin wounds. Exp. Cell Res. 299: 465-475. [Medline]
47. Black, R. A., C. T. Rauch, C. J. Kozlosky, J. J. Peschon, J. L. Slack, M. F. Wolfson, B. J. Castner, K. L. Stocking, P. Reddy, S. Srinivasan, et al 1997. A metalloproteinase disintegrin that releases tumor-necrosis factor- from cells. Nature 385: 729-733. [Medline]
48. Elbashir, S. M., J. Harborth, W. Lendeckel, A. Yalcin, K. Weber, T. Tuschl. 2001. Duplexes of 21-nucleotide RNAs mediate RNA interference in cultured mammalian cells. Nature 411: 494-498. [Medline]
49. Harborth, J., S. M. Elbashir, K. Bechert, T. Tuschl, K. Weber. 2001. Identification of essential genes in cultured mammalian cells using small interfering RNAs. J. Cell Sci. 114: 4557-4565. [Medline]
50. Cheng, G., Z. Cao, X. Xu, E. G. van Meir, J. D. Lambeth. 2001. Homologs of gp91^phox: cloning and tissue expression of Nox3, Nox4, and Nox5. Gene 269: 131-140. [Medline]
51. Lambeth, J. D.. 2002. Nox/Duox family of nicotinamide adenine dinucleotide (phosphate) oxidases. Curr. Opin. Hematol. 9: 11-17. [Medline]
52. Asehnoune, K., D. Strassheim, S. Mitra, J. Y. Kim, E. Abraham. 2004. Involvement of reactive oxygen species in Toll-like receptor 4-dependent activation of NF-B. J. Immunol. 172: 2522-2529. [Abstract/Free Full Text]
53. Park, H. S., H. Y. Jung, E. Y. Park, J. Kim, W. J. Lee, Y. S. Bae. 2004. Cutting edge: direct interaction of TLR4 with NAD(P)H oxidase 4 isozyme is essential for lipopolysaccharide-induced production of reactive oxygen species and activation of NF-B. J. Immunol. 173: 3589-3593. [Abstract/Free Full Text]
54. Sadikot, R. T., H. Zeng, F. E. Yull, B. Li, D. S. Cheng, D. S. Kernodle, E. D. Jansen, C. H. Contag, B. H. Segal, S. M. Holland, et al 2004. p47^phox deficiency impairs NF-B activation and host defense in Pseudomonas pneumonia. J. Immunol. 172: 1801-1808. [Abstract/Free Full Text]
55. Greene, C. M., T. P. Carroll, S. G. Smith, C. C. Taggart, J. Devaney, S. Griffin, S. J. O’Neill, N. G. McElvaney. 2005. TLR-induced inflammation in cystic fibrosis and non-cystic fibrosis airway epithelial cells. J. Immunol. 174: 1638-1646. [Abstract/Free Full Text]
56. Guillot, L., S. Medjane, K. Le-Barillec, V. Balloy, C. Danel, M. Chignard, M. Si-Tahar. 2004. Response of human pulmonary epithelial cells to lipopolysaccharide involves Toll-like receptor 4 (TLR4)-dependent signaling pathways: evidence for an intracellular compartmentalization of TLR4. J. Biol. Chem. 279: 2712-2718. [Abstract/Free Full Text]
57. Sabroe, I., S. K. Dower, M. K. Whyte. 2005. The role of Toll-like receptors in the regulation of neutrophil migration, activation, and apoptosis. Clin. Infect. Dis. 7: (Suppl. 41):S421-S426.
58. Sabroe, I., L. R. Prince, E. C. Jones, M. J. Horsburgh, S. J. Foster, S. N. Vogel, S. K. Dower, M. K. Whyte. 2003. Selective roles for Toll-like receptor (TLR)2 and TLR4 in the regulation of neutrophil activation and life span. J. Immunol. 170: 5268-5275. [Abstract/Free Full Text]
59. Houtmeyers, E., R. Gosselink, G. Gayan-Ramirez, M. Decramer. 1999. Regulation of mucociliary clearance in health and disease. Eur. Respir. J. 13: 1177-1188. [Abstract]
60. Richter, A., R. A. O’Donnell, R. M. Powell, M. W. Sanders, S. T. Holgate, R. Djukanovic, D. E. Davies. 2002. Autocrine ligands for the epidermal growth factor receptor mediate interleukin-8 release from bronchial epithelial cells in response to cigarette smoke. Am. J. Respir. Cell Mol. Biol. 27: 85-90. [Abstract/Free Full Text]
61. Jorens, P. G., J. B. Richman-Eisenstat, B. P. Housset, P. D. Graf, I. F. Ueki, J. Olesch, J. A. Nadel. 1992. Interleukin-8 induces neutrophil accumulation but not protease secretion in the canine trachea. Am. J. Physiol. 263: L708-L713. [Medline]
62. Yoshimura, T., K. Matsushima, S. Tanaka, E. A. Robinson, E. Appella, J. J. Oppenheim, E. J. Leonard. 1987. Purification of a human monocyte-derived neutrophil chemotactic factor that has peptide sequence similarity to other host defense cytokines. Proc. Natl. Acad. Sci. USA 84: 9233-9237. [Abstract/Free Full Text]
63. Sorensen, O. E., D. R. Thapa, A. Rosenthal, L. Liu, A. A. Roberts, T. Ganz. 2005. Differential regulation of -defensin expression in human skin by microbial stimuli. J. Immunol. 174: 4870-4879. [Abstract/Free Full Text]
64. Tjabringa, G. S., J. Aarbiou, D. K. Ninaber, J. W. Drijfhout, O. E. Sorensen, N. Borregaard, K. F. Rabe, P. S. Hiemstra. 2003. The antimicrobial peptide LL-37 activates innate immunity at the airway epithelial surface by transactivation of the epidermal growth factor receptor. J. Immunol. 171: 6690-6696. [Abstract/Free Full Text]

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