3-(4, 5-dimethylthiazole-2-yl)-2, 5-diphenyltetrazolium bromide (MTT) was obtained from Dojindo (Kumamoto, Japan). Poly (dI.dC)-poly (dI.dC) and [γ -³²P] ATP were purchased from Amersham Biosciences UK, Ltd. (Buckinghamshire, England). Collagenase P and recombinant human interleukin (IL)-1β were from Roche Applied Science (Mannheim, Germany). Double-stranded oligonucleotide probes for AP-1 and nuclear factor κB (NF-κB) were purchased from Promega (Madison WI). Rat recombinant platelet-derived growth factor (PDGF)-BB was from R&D Systems (Minneapolis, MN). Rabbit antibodies against phosphospecific MAP kinases, total MAP kinases, and inhibitor of NF-κB (IκB-α ) were purchased from Cell Signaling Technologies (Beverly, MA). Rabbit antibody against glyceraldehyde-3-phosphate dehydrogenase (G3PDH) was from Trevigen (Gaithersburg, MD). HNE, SB203580, SP600125, and U0126 were from Calbiochem (La Jolla, CA). All other reagents were from Sigma-Aldrich (St. Louis, MO) unless specifically described.

All animal procedures were performed in accordance with the National Institutes of Health Animal Care and Use Guidelines. Rat PSCs were prepared from the pancreas tissues of male Wistar rats (Japan SLC Inc., Hamamatsu, Japan) weighing 200-250 g as previously described using the Nycodenz solution (Nycomed Pharma, Oslo, Norway) after perfusion with 0.3 g/L collagenase P[16]. The cells were resuspended in Ham's F-12 containing 100 mL/L heat-inactivated fetal bovine serum (ICN Biomedicals, Aurora, OH), penicillin sodium, and streptomycin sulfate. Cell purity was always more than 90% as assessed by a typical star-like configuration and by detecting vitamin A autofluorescence. All experiments were performed using cells between passages two and five except for those using freshly isolated PSCs. Unless otherwise stated, we incubated PSCs in serum-free medium for 24 h before the addition of experimental reagents.

Cell viability was assessed by the MTT assay as previously described[17]. After treatment with HNE for 24 h, MTT solution was added to the cells at a final concentration of 500 μg/mL and the incubation continued at 37 °C for 4 h. After the incubation period, the medium was aspirated and the formazan product was solubilized with dimethylsulfoxide. Cell viability was determined by the differences in absorbance at wavelengths of 570 min 690 nm.

Intracellular peroxide production was examined as previously described[14]. Briefly, cells were incubated with 2’,7’-dichlorofluorescin diacetate (DCF-DA) at 50 μmol/L for 30 min at 37 °C, and then treated with experimental reagents for an additional 30 min at 37 °C. After chilled on ice, cells were washed with ice-cold PBS, scraped from the plate, and resuspended at 1 × 10 ⁶ cells/mL in PBS containing 10 mmol/L EDTA. The fluorescence intensities of 2’, 7’-dichlorofluorescin formed by the reaction of DCF-DA with peroxides of more than 10000 viable cells from each sample were analyzed by FACSCaliber flow cytometer (Becton Dickinson Co. Ltd., Tokyo, Japan) with excitation and emission settings of 488 and 525 nm, respectively. Prior to data collection, propidium iodide was added to the sample to gate out dead cells. Experiments were repeated at least twice with similar results. The data are expressed as one representative histogram.

Serum-starved PSCs (approximately 80% density) were treated with HNE at the indicated concentrations in the absence or presence of PDGF-BB (25 ng/mL). Cell proliferation was assessed using a commercial kit (Cell proliferation ELISA, BrdU; Roche Applied Science) according to the manufacturer’s instruction. This is colorimetric immunoassay based on the measurement of 5-bromo-2’-deoxyuridine (BrdU) incorporation during DNA synthesis[18]. After 24-hour-incubation with experimental reagents, cells were labeled with BrdU for 3 h at 37 °C, fixed, and incubated with peroxidase-conjugated anti-BrdU antibody. Then the peroxidase substrate 3,3’,5,5’-tetramethylbenzidine was added, and BrdU incorporation was quantitated by differences in absorbance at wavelength 370 min 492 nm.

Nuclear extracts were prepared and electrophoretic mobility shift assay was performed as previously described[19]. Double-stranded oligonucleotide probes for AP-1 (5’-CGCTTGATGAGT CAGCCGGAA-3’) and NF-κB (5’-AGTTGAGGGGACTT TCCCAGGC-3’) were endlabeled with [γ -³²P]ATP. Nuclear extracts (approximately 5 μg) were incubated with the labeled oligonucleotide probe for 20 min at 22 °C, and electrophoresed through a 40 g/L polyacrylamide gel. Gels were dried, and autoradiographed at -80 °C overnight. A 100-fold excess of unlabeled oligonucleotide was incubated with nuclear extracts for 10 min prior to the addition of the radiolabeled probe in the competition experiments.

Luciferase assays were performed as previously described[20] using luciferase expression vectors containing two consensus AP-1 binding sites (TGACTCA), or two consensus NF-κB binding sites (GGGACTTTCC), which were kindly provided by Dr. Naofumi Mukaida (Kanazawa University, Japan). Approximately 1 × 10 ⁶ PSCs were transfected with 2 μg of each luciferase expression vector, along with 40 ng of pRL-TK vector (Promega) as an internal control, using the FuGENE6 reagent (Roche Applied Science). After 24 h, the transfected cells were treated with HNE at 1 μmol/L for an additional 24 h. At the end of the incubation, cell lysates were prepared using Pica Gene kit (Toyo Ink Co., Tokyo, Japan), and the light intensities were measured using a model Lumat LB9507 Luminescence Reader (EG&G Berthold, Bad Wildbad, Germany).

Activation of MAP kinases was examined by Western blot analysis using anti-phosphospecific MAP kinase antibodies as previously described[21]. Cells were treated with HNE, and lysed in sodium dodecyl sulfate buffer (62.5 mmol/L Tris-HCl at pH 6.8, 20 g/L sodium dodecyl sulfate, 100 mL/L glycerol, 50 mmol/L dithiothreitol, 1 g/L bromphenol blue) for 15 min on ice. The samples were then sonicated for 2 s, heated for 5 min, and centrifuged at 12000 g for 5 min to remove insoluble cell debris. Whole cell extracts (approximately 100 μg) were fractionated on a 100 g/L sodium dodecyl sulfate-polyacrylamide gel. They were transferred to a nitrocellulose membrane (Bio-Rad, Hercules, CA), and the membrane was incubated overnight at 4 °C with rabbit antibodies against phosphorylated MAP kinases (extracellular signal-regulated kinase (ERK)1/2, c-Jun N-terminal kinase (JNK), or p38 MAP kinase). After incubation with peroxidase-conjugated goat anti-rabbit secondary antibody for 1 h, proteins were visualized by using an ECL kit (Amersham Biosciences UK, Ltd.). Levels of total MAP kinases, IκB-α , α -SMA, and G3PDH were examined in a similar manner.

After a 24-h incubation, cell culture supernatants were harvested and stored at -80 °C until the measurement. Monocyte chemoattractant protein-1 (MCP-1) levels in the culture supernatants were measured by enzyme-linked immunosorbent assay (Pierce Biotechnology, Rockford, IL) according to the manufacturer's instructions.

PSCs were incubated with HNE in serum-free medium for 48 h. Type I collagen released into the culture supernatant was quantified by enzyme-linked immunosorbent assay, as previously described[22]. Briefly, immunoassay plates (Becton Dickinson, Franklin Lakes, NJ) were coated with diluted samples overnight at 4 °C. After blocking with 50 g/L dry milk in PBS, plates were incubated with goat anti-rat type I collagen antibody (SouthernBiotech, Birmingham, AL). After washing of the plate, rabbit anti-goat IgG antibody conjugated with alkaline phosphatase was added, and incubated. Finally, P-nitrophenylphosphate was added as a substrate, and the collagen levels were determined by differences in absorbance at wavelength 405 min 690 nm. Rat tail collagen type I was used as a standard. The collagen levels in each sample were normalized to the cellular DNA content, which was determined by a fluorometric assay, according to the method of Brunk et al[23]. The results are expressed as a percentage of the untreated control.

Freshly isolated PSCs were incubated with HNE (at 1 μmol/L ) in serum-free medium or 50 mL/L fetal bovine serum-containing medium. After 7-d incubation, morphological changes characteristic of PSC activation were assessed after staining with glial acidic fibrillary protein (GFAP) as previously described[24] using a streptavidin-biotin-peroxidase complex detection kit (Histofine Kit; Nichirei, Tokyo, Japan). Briefly, cells were fixed with 100 mL/L methanol for 5 min at -20 °C, and then endogenous peroxidase activity was blocked by incubation in methanol with 3 mL/L hydrogen peroxide for 5 min. After immersion in normal goat serum for 1 h, the slides were incubated with rabbit anti-GFAP antibody at a dilution of 1:100 overnight at 4 °C. The slides were incubated with biotinylated goat anti-rabbit antibody for 45 min, followed by peroxidase-conjugated streptavidin for 30 min. Finally, color was developed by incubating the slides for several minutes with diaminobenzidine (Dojindo, Kumamoto, Japan). In addition, total cellular proteins (approximately 25 μg) were prepared, and the levels of α -SMA and G3PDH were determined by Western blotting.

The results were expressed as mean ± SD. Luminograms and autoradiograms are representative of at least three experiments. Differences between experimental groups were evaluated by the two-tailed unpaired Student’s t test. A P-value less than 0.05 was considered statistically significant.

Because HNE has been shown to be cytotoxic at high concentrations in several types of cells[25], we first examined the effect of HNE on the cell viability of PSCs. PSCs were incubated with increasing concentrations of HNE for 24 h, and the cell viability was assessed by MTT assay. HNE up to 5 μmol/L did not alter the cell viability, but above 5 μmol/L, HNE was cytotoxic (Figure 1). The results were also confirmed by trypan blue dye exclusion test (data not shown). Based on these results, we used HNE up to 5 μmol/L in the subsequent experiments.

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Figure 1 PSCs were incubated with HNE at the indicated con-centrations in serum-free medium for 24 h. Cell viability was determined by the MTT assay, and the absorbance at 570 min 690 nm (“A.”) of the sample is given. Data are shown as mean ± SD (n = 6). ^aP < 0.05 vs control, ^bP < 0.01 vs control.

We examined the production of pro-oxidants using a peroxide-sensitive fluorescent probe, DCF-DA. This chemical is freely permeable to cells. Once inside the cells, it is hydrolyzed to DCF and trapped intracellularly. In the presence of peroxides, especially hydrogen peroxide, DCF is oxidized to fluorescent 2’,7’-dichlorofluorescin, which can then be readily detected by flow cytometry[14]. Treatment with HNE (at 5 μmol/L) increased the peroxide-activated fluorescence intensity, indicating that HNE was a potential inducer of intracellular oxidative stress in PSCs (Figure 2).

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Figure 2 PSCs were incubated with DCF-DA (at 50 μmol/L ) for 30 min and then treated with HNE (at 1 or 5 μmol/L) for 30 min. The fluorescence intensity of more than 10000 cells was analyzed using a flow cytometer.

We next examined the effects of HNE on the activation of the transcription factors NF-κB and AP-1. These transcription factors are important regulators of gene expression in response to many stimuli including proinflammatory cytokines and growth factors[26,27]. PSCs were incubated with HNE, or IL-1β for 1 h. Nuclear extracts were prepared, and the specific binding activities of AP-1 and NF-κB were examined by electrophoretic mobility shift assay. HNE, as well as IL-1β , increased the AP-1 binding activity (Figure 3A). The specificity of AP-1-specific DNA binding activity was demonstrated by the addition of a 100-fold molar excess of unlabeled AP-1 oligonucleotide, but not by unrelated NF-κB oligonucleotide in competition assays (data not shown). In contrast, NF-κB binding activity was induced by IL-1β , but not by HNE (Figure 3B).

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Figure 3 PSCs were treated with IL-1β (at 2 ng/mL, lane 2) or HNE (at 5 μmol/L, lane 4) in serum-free medium for 1 h. Nuclear extracts were prepared and subjected to electro-phoretic mobility shift assay using AP-1 (panel A) or NF-κB (panel B) oligonucleotide probes. Arrows denote specific in-ducible complexes competitive with cold double-stranded oli-gonucleotide probes (lane 3). Lane 1: control (serum-free medium only). □: free probe.

To confirm that AP-1 activation observed by electrophoretic mobility shift assay was functional, the effect of HNE on AP-1 dependent transcriptional activity was examined. PSCs were transiently transfected with NF-κB- or AP-1-luciferase gene reporter constructs and assayed for the luciferase activity. As shown in Figure 4, HNE increased AP-1-dependent, but not NF-κB-dependent luciferase activity. Phosphorylation and degradation of the inhibitory protein IκB-α , and subsequent dissociation of this protein from NF-κB were thought to be necessary for the activation[26]. We also examined the effect of HNE on the degradation of IκB-α by Western blotting. IL-1β , but not HNE, induced transient degradation of IκB-α , further supporting that HNE did not activate NF-κB (Figure 4B).

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Figure 4 HNE increased AP-1, but not NF-κB, -dependent transcriptional activity. A: PSCs were transfected with the lu-ciferase vectors (2 X AP-1 or 2 X NF-κB) along with pRL-TK vector as an internal control. After 24 h, the transfected cells were treated with IL-1β (at 2 ng/mL) or HNE (at 1 μmol/L ). After another 24-h incubation, intracellular luciferase activities were determined. The data represent mean mean ± SD, calcu-lated from three independent experiments as fold induction compared with the activity observed in control (serum-free medium only, “Con”). ^bP < 0.01 vs control. RLU: relative light units. B: PSCs were treated with IL-1β (at 2 ng/mL) or HNE (at 1 μmol/L) in serum-free medium for the indicated times. Total cell lysates were prepared, and the level of IκB-α was deter-mined by Western blotting.

Induction of the expression of AP-1 components c-Fos and c-Jun by a variety of stimuli such as growth factors and cytokines is mediated by the activation of three distinct MAP kinases: ERK1/2, JNK, and p38 MAP kinase[27,28]. Activation of these kinases occurs through phosphorylation[27,28]. We determined the activation of these MAP kinases in HNE-treated cells by Western blotting using anti-phosphospecific MAP kinase antibodies. These antibodies recognize only phosphorylated forms of MAP kinases, thus allowing the assessment of activation of these kinases. HNE activated these three classes of MAP kinases in a time-dependent manner with peaking around 5 to 15 min (Figure 5).

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Figure 5 PSCs were treated with HNE (at 1 μmol/L) for the indicated times. Total cell lysates (approximately 100 μg) were prepared, and the levels of activated, phosphorylated MAP kinases were determined by Western blotting using anti- phosphospecific antibodies. Levels of total MAP kinases were also determined.

We then examined the effects of HNE on basal and PDGF-induced proliferation. As previously reported[16], PDGF-BB significantly increased proliferation. HNE did not affect either basal or PDGF-BB-induced proliferation of PSCs (Figure 6).

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Figure 6 PSCs were treated with HNE (at 0, 1, or 5 μmol/L ) in the absence or presence of PDGF (at 25 ng/mL) in serum-free medium. After 24-h incubation, cells were labeled with BrdU for 3 h. Cells were fixed, and incubated with peroxidase-conju-gated anti-BrdU antibody. Then the peroxidase substrate 3,3’, 5,5’-tetramethylbenzidine was added, and BrdU incorporation was quantitated by differences in absorbance at wavelength 370 min 492 nm (“A.”, optical density). Data are shown as mean ± SD (n = 6). ^bP < 0.01 versus control (serum-free medium only), N.S.: not significant.

Activated PSCs acquired the proinflammatory phenotype; they might modulate the recruitment and activation of inflammatory cells through the expression of MCP-1[29]. IL-1β induced MCP-1 production, but HNE did not (Figure 7).

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Figure 7 PSCs were treated with IL-1β (2 ng/mL, “IL”) or HNE (at 1 or 5 µmol/L ) in serum-free medium. After 24 h, culture supernatant was harvested, and the MCP-1 level was determined by enzyme-linked immunosorbent assay. Data shown are expressed as mean ± SD (n = 6). ^bP < 0.01 versus con-trol (“Con”, serum-free medium only).

It has been shown that culture-activated PSCs express α -SMA and produce type I collagen. Indeed, α -SMA expression has been accepted as a marker of PSC activation[1], and in situ hybridization techniques showed that α -SMA-positive cells were the principal source of collagen in the fibrotic pancreas[4]. HNE increased the production of type I collagen (Figure 8). Our previous finding that ethanol and acetaldehyde induced collagen production through p38 MAP kinase[30] prompted us to examine the role of MAP kinases in HNE-induced type I collagen production. Thus we employed specific inhibitors to block these pathways. A selective p38 MAP kinase inhibitor SB203580[31], and a JNK inhibitor SP600125[32] decreased type I collagen production. In contrast, U0126, a specific inhibitor of MAP kinase kinase activation and consequent ERK1/2 activation[33], did not affect the collagen production. These results suggested that HNE induced type I collagen production through the activation of p38 MAP kinase and JNK, but not ERK pathway.

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Figure 8 PSCs were treated with HNE (at 1 µmol/L , lane 2) in the absence or presence of SB203580 (at 25 mmol/L , lane 3), SP600125 (at 10 µmol/L, lane 4), or U0126 (at 5 µmol/L, lane 5). After 48-h incubation, type I collagen released into the cultute supernatant was quantified by enzyme-linked immunosorbent assay. The collagen levels in each sample were normalized to the cellular DNA content. The results are expressed as a per-centage of the untreated control (“Con”). Data are shown as mean ± SD (n = 6). ^bP < 0.01 vs control (serum-free medium only, lane 1). ^dP < 0.01 vs HNE only (lane 2).

Finally, we examined whether HNE initiated the transformation of PSCs from quiescent to myofibroblast-like phenotype in culture. Freshly isolated PSCs were incubated with HNE in serum-free medium or 50 mL/L serum-containing medium for 7 d. Morphological changes characteristic of PSC activation were assessed after staining with GFAP. After 7 d, PSCs cultured with 50 mL/L serum showed transformation into cells with a myofibroblast-like phenotype (Figure 9A). In contrast, PSCs treated with HNE were small and circular, with lipid droplets presenting in many cells and slender dendritic processes (Figure 9B), as PSCs treated with serum-free medium only (Figure 9C). In agreement with the morphological changes, significant expression of α -SMA was observed on d 7 in serum-treated PSCs, whereas HNE did not induce α -SMA expression.

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Figure 9 A,B,C: Freshly isolated PSCs were incubated with 50 mL/L serum (panel A), HNE (at 1 µmol/L, panel B), or serum-free medium (panel C) for 7 d. Morphological changes characteristic of PSC activation were assessed after staining with GFAP. Original magnification: × 10 objective. D: Total cell lysates (approximately 25 µg) were prepared from cells treated with serum-free medium (“Cont”), 50 mL/L serum (“FBS”), or HNE (at 1 µmol/L) for 7 d, and the levels of α -SMA and G3PDH were determined by Western blotting.