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RECEPTORS AND SIGNAL TRANSDUCTION

Regulation of ERK1/2 by ouabain and Na-K-ATPase-dependent energy utilization and AMPK activation in parotid acinar cells

Division of Signal Transduction, Department of Medicine, Beth Israel Deaconess Medical Center, Boston, Massachusetts

Submitted 31 March 2008 ; accepted in final form 21 July 2008

	ABSTRACT

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
We previously found that the phosphorylation of ERK1/2 by submaximal concentrations of the muscarinic receptor ligand carbachol was potentiated in rat parotid acinar cells exposed to ouabain, a cardiac glycoside that inhibits the Na-K-ATPase. We now report that this signaling phenomenon involves the prevention of negative regulation of extracellular signal-regulated kinase-1/2 (ERK1/2) that is normally mediated by AMP-activated protein kinase (AMPK). Carbachol increases the turnover of the ATP-consuming Na-K-ATPase, reducing intracellular ATP and promoting the phosphorylation/activation of the energy sensor AMPK. Ouabain blocks the reduction in ATP and subsequent AMPK phosphorylation, which is regulated by the AMP-to-ATP ratio. The ouabain-promoted enhancement of ERK1/2 phosphorylation was not reproduced in Par-C10 cells, an immortalized rat parotid cell line that did not respond to carbachol with an ATP reduction and that employs an upstream AMPK kinase (Ca²⁺/calmodulin-dependent protein kinase kinase, CaMKK) different from that (LKB1) in native cells. In native parotid cells, inhibitory effects of AMPK on ERK1/2 signaling were examined by activating AMPK with 5-aminoimidazole-4-carboxamide-1-β-D-ribofuranoside (AICAR), which is converted to an AMP mimetic but does not alter parotid ATP levels. AICAR-treated cells display increases in AMPK phosphorylation and a reduced phosphorylation of ERK1/2 subsequent to activation of muscarinic and P2X₇ receptors, which promote increases in Na-K-ATPase turnover, but not upon epidermal growth factor receptor activation. These results suggest that carbachol-initiated AMPK activation can produce a negative feedback on ERK1/2 signaling in response to submaximal muscarinic receptor activation and that increases in fluid secretion can modulate receptor-initiated signaling events indirectly by producing ion transport-dependent decreases in ATP.

adenosine 5'-triphosphatase; calmodulin-dependent protein kinase kinase; 5-aminoimidazole-4-carboxamide-1-β-D-ribofuranoside; carbachol; 2',3'-O-(4-benzoylbenzoyl)adenosine 5'-triphosphate

In contrast to the effect of low concentrations of ouabain to initiate ERK1/2 activation and signalplex formation, we found that ouabain (10–1,000 µM) did not produce a large stimulation of ERK1/2 phosphorylation in freshly isolated rat parotid acinar salivary gland cells; however, high concentrations of ouabain potentiated the phosphorylation of ERK1/2 downstream of the stimulation of the parotid muscarinic type 3 receptor (M3R) by submaximal concentrations (3 x 10^–7 and 1 x 10^–6 M) of the ligand carbachol (29). The EC₅₀ of ouabain in enhancing the activation of ERK1/2 by 10^–6 M carbachol was 100 µM, and this was similar to the inhibitor constant (K_i) of ouabain in blocking the Na-K-ATPase enzyme activity of rodent cells that express the ₁-subunit of this enzyme. Ouabain did not appear to exert its effects directly on the activation of the M3R itself or on the coupling of the receptor to phospholipase C, since the IP₃-dependent release of intracellular Ca was not affected in ouabain-treated cells. Src and PKC contributed positively to the activation of ERK1/2 by maximal concentrations of carbachol as well as to the potentiation by ouabain of submaximal carbachol concentrations.

The focus of the present investigation was to determine how ouabain contributed in a positive manner to the activation of ERK1/2 by the carbachol-initiated activation of the M3R in parotid acinar epithelial cells. Muscarinic ligands promote an increase in fluid secretion by these cells that initiates the production of saliva. This process involves the concerted activation of ion channels and other ion transport proteins, including the ATP-dependent Na-K-ATPase (22). This increases the turnover of ATP, and this activates the energy-sensor AMP-activated protein kinase (AMPK) in parotid cells (32). AMPK is a heterotrimeric complex consisting of a catalytic -subunit and regulatory β- and -subunits, and phosphorylation of Thr172 in the kinase domain at the NH₂-terminus of AMPK is required for activation. AMPK is allosterically activated by increases in AMP, and increases in the AMP-to-ATP ratio enhance the phosphorylation of AMPK by the upstream AMPK kinase LKB1 (38). AMPK plays a central role in many metabolic effects, including those involved in insulin signaling as well as responses to stress, and has an inhibitory effect on cell growth, proliferation, and cell survival (20, 38). AMPK has been found to have both positive and negative effects on ERK signaling (4, 7, 16, 17). Since we previously found that carbachol increased AMPK phosphorylation in parotid acinar cells, we examined carbachol-stimulated ERK1/2 signaling more closely to determine whether AMPK and upstream signaling molecules in the ERK1/2 cascade contributed to the potentiation of ERK1/2 phosphorylation by ouabain. Our findings suggest that stimulation of the Na-K-ATPase turnover can dampen the activation of ERK1/2 by carbachol in native parotid acinar cells under some conditions. In parallel experiments, the effects of AMPK on ERK1/2 signaling were examined by activating AMPK with AICAR, a cell-permeable compound that is converted to an AMP mimetic. We compared the effects of AICAR on ERK1/2 phosphorylation by ligands to three different types of receptors, including carbachol (G protein-coupled muscarinic receptors), 2',3'-O-(4-benzoylbenzoyl)adenosine 5'-triphosphate (BzATP; P2X₇ receptors, which also are ion channels), and epidermal growth factor (EGF, growth factor receptors). The results suggest that receptor-mediated Na-K-ATPase-dependent increases in ATP hydrolysis can affect the activities of protein kinases in the ERK1/2 signaling cascade.

We also conducted similar studies using Par-C10 cells, an immortalized cell line of rat parotid acinar cells that share many of the receptor types, second messenger production, cell signaling events, and ion transport characteristics of native rat parotid cells (39). This cell line is also amenable to transfections and alterations of protein expression and ideally could be used for directed studies of the proteins involved in the potentiation of ERK1/2 by ouabain in carbachol-treated cells. However, we were unable to replicate our findings concerning ouabain and ERK1/2 activation. We explored the reasons for the different responses between native and immortalized cells and found this to be due to differences in cell metabolism and the regulation of key signaling molecules, including the kinases upstream of AMPK.

	MATERIALS AND METHODS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Chemicals. Carbamylcholine (carbachol) (C-4382), ATP (A-2383), carbonyl cyanide-p-trifluoromethoxyphenyl hydrazone (FCCP) (C-2920), and ouabain (O-3125) were purchased from Sigma. STO-609 (1551) was obtained from Tocris. Rabbit polyclonal ERK2 (SC-154) and mouse monoclonal ERK2 (SC-1647) were purchased from Santa Cruz Biotechnology. The following phospho-specific antibodies were purchased from Cell Signal Technology: Thr202/Tyr204-ERK1/2 (9101), Ser217/221-MEK (9121), Thr172-AMPK (2532), Ser79-ACC (3661), Ser338-C-Raf (9427), and LKB1 (3052). Ca²⁺/calmodulin-dependent protein kinase kinase (CaMKK) antibody (610544) was purchased from BD Transduction Laboratories. -Isoform-specific (1, -2, and -3) Na-K-ATPase antibodies were provided by Dr. Thomas A. Pressley (Texas Tech University Health Sciences Center). Secondary antibodies used for the Odyssey Infrared Imaging System were IRDye 800 conjugated goat anti-rabbit IgG (Rockland, no. 611-632-122) and Alexa Fluor 680 goat anti-mouse IgG (Invitrogen A-21058). Goat anti-rabbit IgG (AP307P) and goat anti-mouse IgG (AP124P) secondary antibodies used for Western blot analysis using film were obtained from Chemicon. Igepal was purchased from ICN Biomedicals. All other chemicals were reagent grade or better.

Parotid acinar cell preparation. Parotid acinar cells were prepared from male Sprague-Dawley rats (Charles River Laboratories, Kingston, NY, or Taconic, Germantown, NY; 175–225 g) using previously established techniques (34). The Institutional Animal Care and Use Committee of Beth Israel Deaconess Medical Center approved this study. In brief, rat parotid glands were removed and treated with trypsin and collagenase to get a suspension of single cells and small groups of cells. Cells were suspended at 0.5–1 mg protein/ml in solution A composed of the following (in mM: 116.4 NaCl, 5.4 KCl, 1 NaH₂PO₄, 25 Na HEPES, 1.8 CaCl₂, 0.8 MgCl₂, 5 Na β-hydroxybutyrate, and 5.6 glucose, pH 7.4). Cells were maintained on ice before use.

All treatments of cells were performed at 37°C in a water-jacketed chamber using a magnetic flea to stir the suspended cells. Aliquots of cells (usually 1.5 ml) were equilibrated for 10 min before treatment with various agents or vehicles [water or 0.1–0.2% dimethylsulfoxide (DMSO)]. At the end of the treatment period, parotid cells were collected by rapid sedimentation in a microcentrifuge (Brinkmann 5414). The supernatant was removed, and cells were lysed in 500 µl of ice-cold lysis buffer [137 mM NaCl, 20 mM Tris base, pH 7.5, 1 mM EGTA, 1 mM EDTA, 10% (vol/vol) glycerol, and 1% (vol/vol) Igepal] containing the following reagents: 1 mM vanadate, 4.5 mM sodium pyrophosphate, 47.6 mM NaF, 9.26 mM β-glycerophosphate, 0.5 mM dithiothreitol, 2 mg/ml leupeptin, 2 mg/ml pepstatin, 2 mg/ml aprotenin, and 2 mg/ml 4-(2-aminoethyl)-benzenesulfonyl fluoride hydrochloride (AEBSF). The lysates were vortexed extensively and then sedimented at 15,000 g for 15 min at 4°C. The cleared supernatants were transferred to fresh microfuge tubes and diluted with 5x Laemmli sample buffer [312.5 mM Tris·HCl (pH 6.8), 25% glycerol, 5% sodium dodecyl sulfate, 1.8 M β-mercaptoethanol, and bromophenol blue (trace)], boiled for 5 min, and stored at –20°C before electrophoresis.

Par-C10 cells. Cells were grown to near confluence in DMEM-F12 (1:1) medium containing 2.5% fetal bovine serum (FBS) and supplements similar to those specified in Turner et al. (39). Cells were cultured on 100-mm BD Falcon tissue culture dishes in a humidified atmosphere of 95% air-5% CO₂ at 37°C.

Western blot analysis. Samples were separated using SDS-polyacrylamide gel electrophoresis with a 10% separating gel and a 3% stacking gel as described previously (29). Proteins were transferred from the gels to nitrocellulose. Immunoblots were probed overnight with various antibodies according to the supplier's specifications. Proteins were visualized using enhanced chemiluminescence (ECL) reagents and X-ray film; alternatively, in some experiments proteins were visualized and quantified by direct infrared fluorescence using an Odyssey Imaging System (Li-Cor Biosciences). Blots were stripped and reprobed to identify changes in the phosphorylation status of multiple signaling proteins.

Quantification of protein phosphorylation. For most ERK and AMPK studies, the blots were probed for phosphoproteins and total protein levels using various protein-selective primary antibodies, and fluorescent anti-rabbit and anti-mouse antibodies were used for visualization and subsequent quantification using the Odyssey Imaging System, as reported previously (29). The phosphorylation status of mitogen-activated protein kinase kinase (MEK), RAF, and some AMPK and ERK proteins visualized on film using ECL techniques were quantified by densitometry using the ImageJ software program of the National Institutes of Health. Changes in the phosphorylation status of these proteins were evaluated as an indication of changes in their activation status. For each sample, the level of phosphorylated protein was normalized to the total protein level of the signaling protein being analyzed or to total ERK2 to account for gel loading/transfer variations. Changes in protein phosphorylation for various conditions were compared with the phosphorylation status under basal (nonstimulated) conditions in the absence of inhibitors.

Cellular ATP measurements. ATP was measured in parotid acinar cells as described previously (32). In general, cells suspended in solution A were equilibrated for 10 min at 37°C before treatment with various agents or vehicles (water or 0.1–0.2% DMSO), as indicated. ATP was extracted from the cells using 6% perchloric acid (PCA), the acid extract was neutralized using K₂CO₃, and the sample was frozen at –80°C until it was analyzed spectrophometrically in a hexokinase-linked enzyme assay using authentic ATP as a standard. The ATP content of each sample was normalized to the amount of PCA-precipitated protein. Multiple samples (generally 2–4) for each condition were collected from each cell preparation, and the results from one preparation were averaged and treated as n = 1. The numbers of independent experiments are presented for each condition.

For experiments with Par-C10 cells, the medium was switched to DMEM plus 0.1% FBS overnight or several hours before the experiment. ATP was extracted and quantified as for native parotid acinar cells. Multiple samples (generally 2–4) for each condition were collected from each experiment, and the results from one experiment were averaged and treated as n = 1. The numbers of independent experiments are as presented.

Data. Values were calculated as the means ± SE of n number of independent experiments (each n from a different experiment). Differences between control/basal and experimental samples for the accumulated data were evaluated using a Student's t-test. All experiments, including Western blot analyses, were performed at least three different times. Within each experiment designed to quantify changes in protein phosphorylation using the Odyssey system or film densitometry, multiple (duplicate or triplicate) samples of cells were collected for each condition and were subjected to SDS-PAGE. For the quantification of protein phosphorylation, the average of the values obtained for each condition within each individual experiment was treated as n = 1.

	RESULTS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Effect of ouabain on signaling proteins upstream and downstream of ERK1/2. In previous studies we observed that ouabain potentiated the activation of ERK1/2 in rat parotid acinar cells by low concentrations of the muscarinic ligand carbachol (29). The relatively low potency of ouabain on ERK1/2 enhancement suggested that this effect was mediated by the ouabain-binding ₁-subunit, which is known to be ouabain-insensitive in rodents. To examine the -subunit isoforms, we probed parotid gland lysates with isoform-specific antibodies, and found that the parotid gland expresses the ₁-subunit (Fig. 1). Brain tissue expresses all three isoforms and served as a positive control for the antibodies. These results were consistent with the high concentration dependence of ouabain on ERK1/2 potentiation being mediated via the ₁-subunit.

View larger version (22K): [in this window] [in a new window]   Fig. 1. Western blot of 1-, 2-, and 3-subunits of the Na-K-ATPase. 1 was detectible in brain, parotid gland, and a rat parotid cell line (Par-C10). 2 and 3 expression were readily detectible in brain but not in parotid or Par-C10 cells. All lanes were loaded with 100 µg protein.

View larger version (26K): [in this window] [in a new window]   Fig. 2. Ouabain (Ouab) increases the effect of carbachol (Carb) on the phosphorylation of proteins in the extracellular signal-regulated kinase-1/2 (ERK1/2) signaling cascade but blocks AMP-activated protein kinase (AMPK) phosphorylation. A: parotid acinar cells were treated with 10–6 M Carb for 2 min after a 1-min exposure to DMSO (–) or 1 mM Ouab and to 10–5 M Carb after a 1-min exposure to DMSO. Cells in basal (–) condition were exposed for Ouab or DMSO for 3 min. Lysates were subjected to immunoblot analysis as indicated. Representative Western blot analysis of replicate samples from one experiment. Ouab increases the phosphorylation of RAF-S338, mitogen-activated protein kinase kinase (MEK), and ERK1/2 in cells treated with 10–6 M Carb. B: quantification of changes in phosphorylation of ERK1/2, MEK, and RAF. For each condition, the level of phosphoprotein was quantified and normalized to the total individual protein (ERK2, MEK, RAF), and values are presented relative to basal (no Ouab). Number of individual experiments is indicated below bars. *P < 0.02 vs. basal (no Ouab). #P < 0.01 vs. 10–6 M Carb (no Ouab). ##P 0.05 vs. 10–6 M Carb (no Ouab). All other conditions are P 0.01 vs. basal (no ouabain). C: parotid acinar cells were treated with 10–6 and 10–5 M Carb for 2 min after a 1-min exposure to DMSO (–) or 1 mM Ouab. Cells in basal (–) condition were exposed for Ouab or DMSO for 3 min. Lysates were subjected to immunoblot analysis using a P-AMPK antibody. Representative Western blot analysis of replicate samples from one experiment. Ouab reduces/blocks the phosphorylation of AMPK. D: quantification of AMPK phosphorylation. For each condition, the phosphorylation of AMPK was quantified and normalized to total AMPK (or ERK2) as a loading control, and values are shown relative to basal (no Ouab). Number of individual experiments is indicated at base of bars. *P < 0.01; **P < 0.05. P values were calculated based on matched pairs from same experiment.

AMPK activation reduces ERK1/2 phosphorylation. To examine the involvement of AMPK in ERK1/2 activation in a more direct manner, we treated parotid cells with AICAR, a cell-permeable compound that is converted to an AMP mimetic that is used to activate AMPK (42), and we tested its effect on the stimulation of ERK1/2 by various receptor ligands in rat parotid acinar cells. First, we confirmed that AICAR affected AMPK in parotid acinar cells. When cells were exposed to AICAR for 5–15 min (Fig. 3), there was an increase in AMPK phosphorylation, indicating the activation of this kinase. Consistent with this, the phosphorylation of acetyl CoA carboxylase (ACC), a downstream substrate of AMPK, also was increased in AICAR-treated cells. To test the effect of AMPK on ERK1/2 activation, we exposed parotid cells to various stimuli with or without pretreatment with AICAR (Fig. 4). The treatment of cells with AICAR significantly reduced the phosphorylation of ERK1/2 promoted by carbachol and BzATP, which activates P2X₇ receptors in parotid acinar cells. AICAR also reduced the phosphorylation of ERK1/2 promoted by the phorbol ester PMA, but it had no effect on the phosphorylation promoted by the growth factor EGF. To examine the involvement of AMPK in the enhancement of ERK1/2 phosphorylation by ouabain, cells were pretreated with vehicle, ouabain alone, or AICAR followed by ouabain; and subsequently they were treated with vehicle or carbachol (Fig. 5). The ouabain-dependent increases in ERK1/2 phosphorylation in cells exposed to 10^–6 M carbachol were not observed in cells that were pretreated with AICAR. AMPK phosphorylation was reduced in cells exposed to ouabain alone or exposed to carbachol subsequent to ouabain, as observed in previous studies (Fig. 2). In contrast, AMPK phosphorylation was elevated above basal levels when ouabain (+/– carbachol) was added subsequent to AICAR. These results along with those in Fig. 4 suggest that the activation of AMPK by AICAR blocked ERK1/2 activation, and conversely, that the reduction in AMPK activation by ouabain (in the absence of AICAR treatment) contributed to the enhanced phosphorylation of ERK1/2 by 10^–6 M carbachol in the presence of ouabain.

View larger version (14K): [in this window] [in a new window]   Fig. 3. 5-Aminoimidazole-4-carboxamide-1-β-D-ribofuranoside (AICAR) increases the phosphorylation of AMPK and acetyl CoA carboxylase (ACC) in parotid acinar cells. A: representative Western blot analysis of parotid acinar cells exposed to 2 mM AICAR for 5–15 min. In one panel the blot was exposed to P-AMPK antibody (long) for an extended period of time. AICAR did not have a consistent affect on AMPK levels. B: quantification of AMPK phosphorylation in cells treated with 2 mM AICAR as indicated. For each condition, the phosphorylation of AMPK was quantified and normalized to total ERK2, and values were calculated relative to basal (no AICAR). n = 3 experiments. P 0.05.

View larger version (17K): [in this window] [in a new window]   Fig. 4. Effects of AICAR on ERK1/2 phosphorylation in parotid cells exposed to different stimuli. Cells were pretreated with AICAR (2 mM) or vehicle for 10–15 min and then exposed to Carb (10–5 M), 2',3'-O-(4-benzoylbenzoyl)adenosine 5'-triphosphate (BzATP, 10 µM), phorbol 12-myristate 13 acetate (PMA, 100 nM), and epidermal growth factor (EGF, 100 µg/ml) for 2 min. A: representative Western blot analysis of different samples from one experiment. Blot was probed with P-ERK1/2 and ERK2 antibodies. B: quantification of ERK1/2 phosphorylation. For each condition, the phosphorylation of ERK1/2 was quantified and normalized to total ERK2, and values are shown relative to basal (no AICAR). AICAR had an inhibitory effect on all stimuli except EGF. Number of individual experiments is indicated at base of bars. *P < 0.01; #P < 0.03.

View larger version (18K): [in this window] [in a new window]   Fig. 5. AICAR blocks the action of ouabain to increase ERK1/2 phosphorylation by 10–6 M Carb. Cells were pretreated with AICAR (2 mM, 10–15 min) before exposure to 10–6 M Carb for 2 min. Cells were treated with ouabain (1 mM) for 1 min before Carb where indicated; cells were exposed to ouabain for 3 min if Carb was not added. A: blot was probed with P-ERK1/2, ERK2, and P-AMPK antibodies. Representative Western blot analysis of samples collected from one experiment. Vertical line indicates location on immunoblot in which nonrelevant samples were excised. B: quantification of ERK and AMPK phosphorylation from multiple experiments. Number of individual experiments shown at bottom of bars. *P 0.05 vs. basal (no additions). **P < 0.01 vs. basal (no additions). #P < 0.01 vs. Carb + Ouab.

View larger version (24K): [in this window] [in a new window]   Fig. 6. Ouabain does not block the stimulation of AMPK phosphorylation or enhance ERK1/2 phosphorylation in Carb-treated Par-C10 cells. Cells were pretreated with 1 mM ouabain or vehicle (DMSO) for 2 min before exposure to 10–4–10–7 M concentrations of Carb (3 min). Samples were lysed and subjected to SDS-PAGE electrophoresis. For each condition, the phosphorylations of ERK1/2 and AMPK were quantified and normalized to total ERK2 and are shown relative to basal (no Ouab). N = 4 for all values, except n = 3 for 10–4 M Carb. At all concentrations of Carb, the comparison between control and ouabain-treated cells were not statistically different.

View larger version (21K): [in this window] [in a new window]   Fig. 7. Relative levels of CaMKK and LKB1 in Par-C10 and native parotid acinar cells. Lysates (50 µg/lane) of each cell type were subjected to Western blot analysis and probed with CaMKK and LKB1 antibodies. Native cells have much more LKB1 protein than Par-C10 cells, and Par-C10 cells have more CaMKK protein than native cells.

View larger version (15K): [in this window] [in a new window]   Fig. 8. STO-609 blocks the stimulation AMPK phosphorylation but not ERK1/2 phosphorylation in Par-C10 cells. Cells were pretreated with various concentrations of the CaMKK inhibitor STO-609 for 60 min and then exposed to 10–4 M Carb (3 min). Samples were lysed and subjected to SDS-PAGE electrophoresis. For each condition, the phosphorylations of ERK1/2 and AMPK were quantified and normalized to total ERK2 levels and are shown relative to control (no STO-609). Number of individual experiments is indicated at base of bars. *P < 0.01 vs. basal (no STO-609); **P < 0.01 vs. carbachol (no STO-609).

View larger version (14K): [in this window] [in a new window]   Fig. 9. Ouabain blocks the Carb-promoted decrease of the cellular ATP content of rat parotid acinar cells. Cells were pretreated with DMSO or ouabain (1 mM) for 1 min and then treated with vehicle (basal) or 10–6 and 10–5 M carbachol for 2 min. Other cells were treated with AICAR (2 mM, 15 min) and FCCP (10 µM, 2 min). In each experiment, the ATP contents were calculated relative to the basal (no Ouab) content (4.5 ± 0.3 nmol ATP/mg protein, n = 6). Number of individual experiments is indicated at base of bars. *P < 0.01 vs. basal (no ouabain); **P 0.02 vs. basal (no Ouab).

Recently, it was suggested that AICAR itself can have negative effects on mitochondrial oxidative phosphorylation and can activate AMPK in some cells by reducing ATP and changing adenine nucleotide levels (9). To investigate this, we exposed rat parotid acinar cells to AICAR (2 mM, 15 min) and examined the ATP levels. Under these conditions AICAR did not produce any significant change (Fig. 9), suggesting that it did not activate AMPK indirectly by decreasing ATP levels.

	DISCUSSION

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
The present study was based on previous experiments indicating that inhibition of the Na-K-ATPase by ouabain potentiated the activation of ERK1/2 in parotid cells exposed to low concentrations of carbachol. In new studies we observed the following: 1) ouabain enhanced the actions of carbachol on the phosphorylation of MEK and C-RAF, kinases that are immediately upstream of ERK1/2; 2) carbachol promotes an increase in AMPK phosphorylation and this is reduced in cells exposed to ouabain; 3) ouabain blocks the carbachol-promoted decreases in cellular ATP levels; 4) the activation of AMPK by AICAR reduces the phosphorylation of ERK1/2 in response to carbachol and BzATP, ligands to parotid M3 and P2X7 receptors, respectively, that increase the Na-K-ATPase turnover; and 5) ouabain did not enhance the phosphorylation of ERK1/2 by carbachol in cells in which AMPK was preactivated by AICAR. These data suggest that AMPK is activated by the enhanced energy utilization (ATP consumption) by the Na-K-ATPase in carbachol-treated cells, and that under some conditions this produces an ouabain-sensitive negative effect on ERK1/2 activation.

In previous studies (29) we investigated whether ouabain itself promoted a substantial increase in ERK1/2 signaling in freshly dispersed parotid acinar cells in the manner in which it does in many cultured epithelial and nonepithelial cells. Although ouabain produced a modest increase in ERK1/2 phosphorylation in parotid cells within several minutes, there was generally less than a 50% increase in the basal state of ERK1/2 phosphorylation (as in Fig. 2B), and this required large ouabain concentrations. In contrast, low ouabain concentrations (10 µM) are often sufficient to activate ERK1/2 in many cell lines or primary cells in culture. This response to ouabain involves the Na-K-ATPase -subunits serving as signaling receptors/signalplexes that are localized in caveolae, where they associate with many signaling proteins (23, 28, 37). Recently, it was shown that there are two pools of Na-K-ATPase proteins in the plasma membrane of LLC-PK1 (pig kidney) cells. One pool is the ion pumping and energy-transducing enzyme, and the other is the signaling protein (19).

The Na-K-ATPase is made up of a heterodimer of an -subunit, which binds ouabain, and a β-subunit, and there are multiple isoforms of each subunit (2). In some systems, a -subunit can act in a regulatory manner (36). Many cells in which low concentrations of ouabain promote signal transduction events have an -subtype with a high sensitivity (low micromolar or less) to ouabain for ion transport inhibition as well as cell signaling. Differences in ouabain sensitivity can be due to different -isoforms as well as to differences among species. The different sensitivities of pig (LLC-PK1) and rat (A75R) cells responding to the activation of ERK and Src by ouabain were also observed for its effects on Na-K-ATPase inhibition: pig cells were 100 times more sensitive for both signaling and Na-K-ATPase inhibition (10), However, the K_i (100 µM) of a rat ₁/β₁ dimer is 100-fold less sensitive to ouabain than rat ₂- and ₃-subunits paired in different combinations with β₁ and β₂ (2). Nonetheless, even in cultured rat cells, very low (10–100 nM) concentrations of ouabain were sufficient to promote Ca²⁺ oscillations (1) and to activate ERK and promote cell growth (6) at concentrations that did not produce significant increases in intracellular Na due to Na-K-ATPase inhibition. In contrast, in primary cultures of rat myocytes, ERK activation and PKC translocation was promoted by a concentration of ouabain (100 µM) that blocked about 50% of the ion transporting activity of the Na-K-ATPase (24). The rat specificity of ouabain signaling to ERK was examined by expressing rat β₁ and different rat -isoforms in insect sf9 cells (27). The ₁/β₁-isozyme was 100–1,000-fold less sensitive than ₃/β₁- and ₄/β₁-, and ₂/β₁-isozymes did not respond to ouabain,. Rat parotid gland expresses primarily the ouabain-insensitive ₁-isoform (Fig. 1). Recently, very low mRNA levels of the ₂-isoform also were detected in rat parotid glands using quantitative PCR (18).

These studies were designed to investigate how the Na-K-ATPase inhibitor ouabain acted in concert with carbachol to enhance the activation of ERK1/2. Unlike most studies of ouabain on signaling events, the potentiation by ouabain of ERK1/2 phosphorylation in cells treated with 10^–6 M carbachol was dependent on its inhibition of the Na-K-ATPase enzyme activity, since the effects of ouabain on ERK signaling and Na-K-ATPase inhibition both displayed similar concentration dependencies (29). Our new findings suggested that this involves AMPK, an energy sensor that responds to agents that alter the AMP-to-ATP ratio (12, 38) and which can negatively affect ERK1/2 activation in some cells. In fact, the inhibitory effect of AICAR on the M3R-promoted increases in ERK1/2 phosphorylation (Fig. 4) suggested that activated AMPK can block ERK1/2 activation downstream of this receptor in parotid cells. Moreover, since ouabain blocked the decrease in ATP (Fig. 9) and the increase in AMPK phosphorylation (Fig. 2) promoted by carbachol, this suggested that AMPK was activated by the alteration of ATP and other nucleotides subsequent to the increases of the Na-K-ATPase turnover that accompany increases in fluid secretion/saliva formation. Thus the data suggest that by preventing AMPK activation by 10^–6 M carbachol, ouabain blocked an inhibitory effect of AMPK on ERK1/2. These findings suggest that that AMPK can have a central role in the regulation of ERK1/2 activation under physiological conditions that are related to the relatively high energy demands necessary to support ion movement, which is accompanied by large increases in oxidative phosphorylation in salivary and other epithelial cells (21, 25, 34). We have interpreted our data in terms of the tight coupling between the Na-K-ATPase and mitochondria for the replenishment of ATP utilized to support ion movement in many types of epithelial tissues (21). However, in rat submandibular salivary glands, the creatine phosphokinase system also may be involved in the replenishment of ATP from phosphocreatine during rapid energy utilization when fluid secretion is stimulated (26). Under such conditions, creatine phosphate could indirectly modulate AMPK activity, as has been suggested upon skeletal muscle contraction (35).

The effectiveness of AICAR in negatively regulating ERK1/2 activation in parotid acinar cells downstream of both the P2X₇ ion channel/receptor and the G protein-coupled muscarinic receptor (Fig. 4) is consistent with our observations that these two diverse receptor types activate similar signaling molecules and cascades including those leading to ERK1/2 (3). Related to this, the inhibitory effect of AICAR on ERK1/2 phosphorylation promoted by PMA, which activates PKC family members in parotid and other cells, also is consistent with previous findings that PKC contributes to ERK1/2 activation by both M3 and P2X₇ receptors (3). Carbachol and BzATP also both increase the Na-K-ATPase turnover in parotid cells (33). Previously, we (32) observed that there was an increase in AMPK phosphorylation in parotid cells exposed to carbachol and BzATP and to mitochondrial uncouplers. Ouabain blocked the phosphorylation promoted by the receptor ligands but not by the uncouplers, since the reductions in ATP promoted by the latter were not due to activation of the Na-K-ATPase. Of interest, the increases in cellular ATP produced by ouabain in secretory epithelia, such as parotid cells (Fig. 9), as well as in absorptive epithelia (40) attest to the common nature of the large demand that the Na-K-ATPase makes on ATP.

The involvement of AMPK in ERK1/2 activation was selective for the particular stimulating agent, since AICAR did not block EGF-promoted ERK1/2 phosphorylation. Other investigators also reported that AICAR was ineffective in blocking ERK1/2 activation by EGF, although it did block the stimulation by IGF-1 at the level of Ras (16). Activation of AMPK by AICAR also blocked ERK activation by serum in cultured rat cardiac fibroblast (7). In contrast, AICAR increased ERK activity in rat muscle (4) and promoted the phosphorylation of ERK1/2 in an AMPK-dependent manner in HepG2 cells (41), a phenomenon that we did not observe in parotid acinar cells (Fig. 4). In liver cells AICAR lowered ATP levels by blocking oxidative phosphorylation in an AMPK-independent manner (9). AICAR did not have this effect on parotid cells, since it did not lower ATP levels (Fig. 9). Potentially, such an action would have a negative effect on the Na-K-ATPase in an indirect manner (i.e., ATP limitation). However, AMPK also could have a more direct role in modifying salivary secretion under various conditions, including metabolic stress, hypoxia, and cellular work. Various ion transport systems, including the cystic fibrosis transmembrane conductance regulator (CFTR), epithelial Na channel (ENaC), and others, can be downregulated via AMPK when energy levels decline in cells (11).

A schematic model of the effect of ouabain on signaling in rat parotid acinar cells stimulated with carbachol is shown in Fig. 10. Carbachol stimulates G protein-coupled M3 muscarinic receptors linked to phospholipase C, generating diacylglycerol and second messengers that increase intracellular Ca²⁺ concentration ([Ca²⁺]_i). The rise in [Ca²⁺]_i opens ion channels and stimulates other ion transporters that increase intracellular Na and reduce intracellular K, thereby activating the Na-K-ATPase and leading to an increase in ATP hydrolysis and the activation of AMPK. The production of second messengers also leads to the activation of ERK1/2 in a cascade that involves MEK and C-RAF activation. When cells are exposed to low (<10^–5 M) concentrations of carbachol, the stimulation of AMPK dampens the activation of ERK1/2, probably acting at a level of C-RAF or above. This inhibitory effect can be blocked by ouabain, which blocks AMPK activation by blocking the increased consumption of ATP by the Na-K-ATPase.

View larger version (9K): [in this window] [in a new window]   Fig. 10. Schematic model of the effect of ouabain on signaling in rat parotid acinar cells treated with carbachol. Carbachol stimulates the G protein-coupled M3 muscarinic receptor, generating second messengers that initiate the ERK1/2 activation cascade (right). Carbachol also promotes ionic alterations that increase the Na-K-ATPase activity, which increases ATP hydrolysis and the activation of AMPK, which can have inhibitory effects on ERK1/2 activation under some conditions. Ouabain inhibits ATP hydrolysis by the Na-K-ATPase, thereby indirectly blocking AMPK activation. AMPK can also be activated by AICAR, which also blocks ERK1/2 activation. See text for more details.

We employed Par-C10 cells in an attempt to duplicate the ouabain studies in a cell culture system that could be manipulated and evaluated by molecular approaches. However, relevant components of the signaling effects observed in native parotid cells were not obtained in these cells: ouabain did not enhance the effects of low concentrations of carbachol on ERK1/2 phosphorylation, carbachol did not alter the ATP content, and ouabain did not block increases in AMPK phosphorylation promoted by carbachol. Differences in the cellular responses in native and PAR-C10 cells were due to various factors. Perhaps the foremost difference is that of cell metabolism, which is oxidative in native cells and likely glycolytic in Par-C10 cells, consistent with the relative differences in the actions of mitochondrial uncouplers on ATP in the two parotid cell types. Also, the density of the Na-K-ATPase ₁-protein is much less in Par-C10 cells compared with native parotid acinar cells (Fig. 1). Finally, AMPK activation in Par-C10 cells appears to be due to the activation of CaMKK (Fig. 8) rather than LKB1, which is found in much lower levels in Par-C10 cells than in native cells (Fig. 7). These findings demonstrate that there are important differences between native and immortalized parotid cells regarding the regulation of key signaling molecules.

Although the rationale for our studies was to an attempt to understand how ouabain enhanced the effects of carbachol on ERK1/2 phosphorylation, our results also suggest a novel way that intrinsic metabolic aspects of cell functions can regulate signaling downstream of receptor activation in some cells. This new paradigm potentially has a more widespread application and greater significance to signaling biology than simply offering an explanation of our previous findings. Although numerous studies have documented how metabolic events can affect signaling by insulin and other growth factors and hormones, far fewer studies have described cell signaling interactions involving a cast of receptors, oxidative metabolism, and ion transport proteins. The data presented here offer new details to explain functional signaling links between the Na-K-ATPase and ERK1/2 that involve metabolic changes that are initiated when fluid secretion is initiated or modified. As demonstrated here for ERK1/2, the energy utilization by the Na-K-ATPase can impose a unique regulation of cell signaling and this doubtlessly has biological ramifications.

	GRANTS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
This work was supported by the National Institute of Dental and Craniofacial Research Grant DE-10877.

	ACKNOWLEDGMENTS

 
We thank Bin Zheng and Atsuo Sasaki (Beth Israel Deaconess Medical Center) for helpful comments and discussions. We also thank David Quissell (University of Colorado Health Sciences Center, Boulder) and Jean Camden (University of Missouri, Columbia) for providing Par-C10 cells. We thank Thomas A. Pressley (Texas Tech University Health Sciences Center) for generously providing antibodies to the Na-K-ATPase -subunits.

	FOOTNOTES

 

Address for reprint requests and other correspondence: S. P. Soltoff, Beth Israel Deaconess Medical Center, New Research Bldg. Rm. 1030-J, 77 Ave. Louis Pasteur, Boston, MA 02111 (e-mail: ssoltoff{at}bidmc.harvard.edu)

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

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