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Dopamine Regulates NA,K-Adenosine Triphosphatase in Alveolar Epithelial Cells via the Mitogen-Activated Protein Kinase/Extracellular-Signal-Regulated Kinase Pathway^*

^* From the Division of Pulmonary and Critical Care Medicine, Michael Reese Hospital, University of Illinois at Chicago, Chicago, IL, and National Cancer Institute, National Institutes of Health, Bethesda, MD.

Correspondence to: J.I. Sznajder MD, FCCP, Department of Medicine, Michael Reese Hospital and Medical Center, 2929 S Ellis Ave, Baum-101, Chicago, IL 60616

Alveolar epithelial Na,K-adenosine triphosphatase (ATPase) plays an important role in lung edema clearance.¹ Na,K-ATPase is an integral membrane protein consisting of the subunit, which has catalytic activity and ion binding sites,² and the ß subunit, which plays a regulatory role contributing to the stability of the complex and its insertion in the plasma membrane.³ Dopamine (DA) upregulates the Na,K-ATPase in the alveolar epithelium and increases lung liquid clearance,⁴ but the mechanisms of this regulation have not been elucidated. The mitogen-activated protein kinase (MAPK), also known as extracellular-signal-regulated kinase (ERK) cascade, is a major signaling system by which cells transduce extracellular signals into intracellular responses.⁵ In mammalian cells ERK proteins, ERK1 and ERK2, also known as p44/p42 respectively, are activated by a variety of hormones, growth factors, and peptides.⁶ Little is known about ERK activation by catecholamines and we are not aware of studies about ERK activation in alveolar type II (ATII) cells. Thus, we tested whether ERK proteins are activated by DA in ATII cells and whether this activation is involved in the upregulation of the Na,K-ATPase in these cells.

Experimental Design and Results

ATII cells were isolated from adult pathogen-free Sprague Dawley male rats (weight approximately 225 g) using the method by Dobbs et al.⁷ Total cellular RNA from ATII cells was isolated by using RNeasy total RNA kit (QIAGEN; Valencia, CA), as described by the manufacturer. The reverse transcriptase reaction was performed (using the Superscript Preamplification System) (GIBCO-BRL; Grand Island, NY) and G3PDH was used as control in the polymerase chain reaction reactions. Western Blot analysis with total protein was performed using the ECL-plus detection kit (Amersham) as recommended by the manufacturer. For determination of the ERK activity, the cells were starved for 16 to 20 h prior to treatment with agonists and antagonists. The ERK activity was determined as described in the "p44/p42 MAP kinase assay kit manual" (New England Biolabs).

Incubation of ATII cells with 1 µM DA resulted in a rapid stimulation (within 2 to 10 min) of ERK activity, measured as phosphorylation of the ERK substrate Elk-1. To study whether the activation of ERK proteins by DA plays a role in the regulation of the Na,K-ATPase, subconfluent day 2 ATII cells were serum starved and treated with the following: (1) control; (2) 1 µM DA; and (3) 50 µM of the specific MEK inhibitor PD98059, 2 h prior to DA stimulation, at times ranging between 1 and 30 h. RT-polymerase chain reaction analysis of total RNA showed that, while the ₁-messenger RNA (mRNA) levels did not change significantly in the DA-stimulated cells, there was an increase in the ß₁-mRNA levels after 6 h of DA stimulation that was maximal between 12 and 18 h. This increase was mediated by ERK activation, as the MEK inhibitor PD98059 completely blocked the DA-induced increase in ß₁-mRNA. Western blot analysis of ATII cell homogenates showed that Na,K-ATPase ß₁-subunit protein increased between 24 and 30 h, following DA stimulation. As with the ß₁ mRNA, the increase in ß₁ protein was inhibited in the presence of the MEK inhibitor PD98059.

To determine which dopaminergic receptor mediates the activation of ERK by DA in ATII cells, we treated the cells with specific agonists and antagonists of the D1 and D2 receptors. Our results showed that D2 but not D1 antagonists blocked the DA activation of ERK proteins. Moreover, inhibition of D1 receptors resulted in a further increase in ERK activation by DA. These results indicate that D2 receptors are involved in the DA-mediated ERK activation and that D1 receptors activation has actually an antagonistic effect on the ERK activation.

Ras proteins are membrane-bound guanine nucleotide-binding proteins that mediate ERK activation in different cell types.⁸ To determine whether Ras proteins are involved in the ERK activation by DA, ATII cells were treated with a peptide corresponding to the SH3 binding sequence of the Ras guanine nucleotide exchange factor SOS (Calbiochem). The SH3-binding region of SOS has strong affinity for the N-terminal SH3 domain of the adaptor protein Grb2⁹ blocking the interaction SOS/Grb2 and thereby preventing Ras activation. Preincubation of ATII cells with the SH3-binding peptide, 10 to 20 µM prior to DA stimulation did not block ERK activation by DA. Under the same conditions, ERK activation by epidermal growth factor was completely blocked in the presence of the SH3-binding peptide. These results suggest that the DA-mediated ERK activation in ATII cells is a Ras-independent mechanism.

Raf1 is a ser/thr kinase that participates in ERK activation.⁶ Although Raf1 is a Ras efector, it can be activated by a Ras-independent mechanism.⁸ To determine whether Raf1 kinase is involved in the DA-mediated ERK activation in ATII cells, we performed a Raf1 assay on cells treated with DA, using syntide-2 as substrate.¹⁰ Our results show that DA stimulated Raf1 kinase activity in ATII cells and that this activation was Ras independent. The involvement of Raf1 kinase in the DA-ERK pathway was confirmed by treatment of the cells with forskolin, a protein kinase A activator, as forskolin completely blocked the activation of ERK by DA. Treatment with the protein kinase A inhibitor adenosine-3', 5'-cyclic monophosphothioate showed the opposite effect.

It has been shown that ERK proteins can be activated by protein kinase C (PKC) and be mediators of the multiple effects of PKC, such as differentiation and proliferation.¹¹ To investigate whether PKC is a component of the signal transduction pathway DA-ERK, we treated ATII cells with the PKC inhibitors bisyndolilmaleimide (1 µM) and calphostin-C (100 nM) prior to DA stimulation. We observed that bisindolylmaleimide blocked the activation of ERK by DA, whereas calphostin-C, an inhibitor of diacylglycerol-dependent PKC isoforms, did not inhibit the stimulation of ERK by DA, suggesting that atypical PKC isoforms may be involved in the DA-ERK pathway in ATII cells.

Discussion

Previous studies have demonstrated that DA increases lung liquid clearance by upregulating the Na,K-ATPase.⁴ Our data suggest that Na,K-ATPase upregulation can be due in part to increased synthesis of the Na,K-ATPase, via a mechanism that involves activation of MAPK/ERK proteins. In the present study, we have in part elucidated a pathway involved in the DA stimulation of ERK activity in ATII cells, which includes D2 receptors, Raf1 kinase, and atypical PKC but is independent of Ras activation.

Our results suggest the existence of a novel pathway of activation of ERK/MAPK in ATII cells. Conceivably, this pathway is an important mechanism in the DA-mediated transcriptional/translational regulation of the Na,K-ATPase in ATII cells and thus, lung edema clearance.

Footnotes

Supported in part by grants HL-48129, American Heart Association grant 96012890, NRSA (KMR), and the Research and Education Foundation of the Michael Reese Medical staff.

References

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2. Cantley, LC (1981) Structure and mechanism of the Na,K-ATPase. Curr Top Bionerget 11,201-237
3. Ackermann, U, Geering, K (1990) Mutual dependence of Na,K-ATPase alpha and beta subunits for correct posttranslation processing and intracellular transport. FEBS Lett 269,105-108
4. Barnard, ML, Olivera, W, Rutschman, DH, et al (1997) Dopamine stimulates sodium transport and lung liquid clearance in rats. Am J Respir Crit Care Med 156,709-714
5. Blenis, J (1993) Signal transduction via the MAP kinases: proceed at your own RSK. Proc Natl Acad Sci USA 90,5889-5892
6. Marshall, CJ (1994) MAP kinase kinase, MAP kinase kinase and MAP kinase. Curr Opin Genet Dev 4,82-89
7. Dobbs, LG, Williams, MC, Gonzalez, R (1988) Monoclonal antibodies specific to apical surfaces of rat alveolar type II cells binds to surfaces of cultured, but not freshly isolated, type II cells. Biochim Biophys Acta 970,146-156
8. Burgering, BMT, Bos, JL (1995) Regulation of Ras-mediated signalling: more than one way to skin a cat. Trends Biochem Sci 20,18-22
9. Li, N, Batzer, A, Daly, R, et al (1993) Guanine-nucleotide-releasing factor hSos1 binds to Grb2 and links receptor tyrosine kinases to Ras signalling. Nature 363,85-88
10. Schramm, K, Niehof, M, Radziwill, G, et al (1994) Phosphorylation of c-RAF-1 by protein kinase A interferes with activation. Biochem Biophys Res Commun 201,740-747
11. van Biesen, T, Hawes, BE, Raymond, JR, et al (1996) G(o)-protein alpha-subunits activate mitogen-activated protein kinase via a novel protein kinase C-dependent mechanism. J Biol Chem 271,1266-1269

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