Dopamine Stimulates Sodium Transport and Liquid Clearance in Rat Lung Epithelium

Dopamine Stimulates Sodium Transport and Liquid Clearance in Rat Lung Epithelium

MICHELE L. BARNARD, WALTER G. OLIVERA, DAVID M. RUTSCHMAN, ALEJANDRO M. BERTORELLO, A. I. KATZ, and JACOB I. SZNAJDER

Columbia Michael Reese Hospital and Medical Center, Pulmonary and Critical Care Medicine and University of Illinois at Chicago, Pulmonary and Critical Care Medicine, Northeastern Illinois University, Department of Mathematics, Chicago, Illinois; Karolinska Institute, Stockholm, Sweden; Department of Medicine, University of Chicago Pritzker School of Medicine, Chicago, Illinois

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Pulmonary edema clearance is driven primarily by active sodium transport out of the alveoli, mediated predominantly by apicalsodium channels and the basolateral NA,K-ATPase. We postulatedthat dopamine, analogous to its effects in other transportingepithelia, could regulate these sodium transport mechanisms andaffect lung liquid clearance. We therefore studied the effectsof dopamine on sodium transport and liquid clearance in isolatedperfused rat lungs. Instillation of dopamine into the airwayscaused a dose-dependent increase in liquid clearance from isolatedrat lungs of up to 33% above control values at 10⁸ to 10⁴ M concentrations. 10⁶ M amiloride, which selectively inhibits apical sodium channels,decreased basal liquid clearance by 34% but did not inhibit thedopamine-mediated stimulation of lung liquid clearance. Instillationof 10⁴ M amiloride into rat airways, which inhibits other sodium transportmechanisms non-selectively, decreased basal lung liquid clearanceby 49% and inhibited the dopamine-mediated stimulation of lungliquid clearance. Perfusion of rat lungs with 5 × 10⁴ M ouabain to specifically inhibit Na,K-ATPase reduced both basalclearance (by 55%) and the dopamine-stimulated increase in lungfluid clearance. Conceivably, the stimulation of lung liquid clearanceby dopamine is due to a modulation of Na,K-ATPase in the pulmonaryepithelium.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The study of pulmonary edema and its pathologic effects has for some time centered on determining mechanisms affecting theformation of alveolar edema, and consequently devising potentialways to prevent accumulation of fluid within the alveolar space.A more likely clinical scenario, however, involves treatment ofpatients who have already developed pulmonary edema. It has beendemonstrated recently that the alveolar epithelium is capableof actively reabsorbing fluid from the alveolar space, and thatthis occurs following actively generated sodium gradients by meansinvolving entry of sodium via apical sodium channels and its extrusionthrough active basolateral transport (1). The latter is principallydriven by the activity of the sodium pump, Na,K-ATPase, whichtransports three Na⁺ ions out of cells and two K⁺ ions into cells at the expense of energy derived from ATP (5).Importantly, this ability of the lungs to clear fluid appearsto be regulated by a number of mechanisms, whose elucidation mightlead to improved clinical management of respiratory failure dueto pulmonary edema.

A large body of information has accumulated regarding regulation of sodium transport in the kidney (6), but much less isknown about other transporting epithelia, notably the alveolarepithelium of the lung. A recent focus of our laboratory and othershas been the short-term regulation of the sodium pump in the alveolarepithelium (10) and specifically, the ability of dopamine toregulate lung liquid clearance.

Catecholamines, both exogenous (in particular $beta$ -adrenergic agonists such as terbutaline or isoproterenol) and endogenous,have previously been shown to increase sodium channel and Na,K-ATPaseactivity in pulmonary alveolar epithelium and to stimulate lungedema clearance (14). We therefore hypothesized that dopaminecould accelerate sodium transport and lung edema clearance inthe isolated perfused rat lung model, and report herein the resultsof this investigation.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Isolated Perfused Lungs

The isolated perfused lung preparation used in our laboratory has been described in detail (3, 4, 11). Briefly, lungsare isolated from anesthetized rats following a 10-minute ventilationwith 100% O₂. The diffusive absorption of oxygen facilitates thefilling of alveoli with instillate fluid. The pulmonary arteryand left atrial appendage are cannulated and perfused with a solutionof 3% bovine serum albumin (BSA) in buffered physiological saltsolution. Fluorescein-labeled (FITC-) albumin is added to theperfusate to monitor leakage of protein from the vascular spaceinto the airways. The recirculating volume of the constant-pressureperfusion system is 90 ml; arterial and venous pressures are setat 12 and 0 cm H₂O, respectively. The lungs are excised from thethoracic cavity and placed in a "pleural" bath (100 ml) filledwith the same BSA solution. The entire system is maintained at37° C in a water bath. The lungs are then instilled via the trachealcatheter with 5 ml BSA containing Evans blue dye-labeled (EBD-)albumin, ²²Na⁺, and ³H-mannitol. Samples are taken from the instillate, perfusate,and bath solutions following a ten-minute equilibration periodand 60 minutes later. Absorbance at 620 nm (for EBD-albumin),fluorescence (excitation 487 nm; emission 520 nm; for FITC-albumin),and scintillation counting (for ²²Na⁺ and ³H-mannitol) are measured in centrifuged samples from each compartment.The EBD-albumin remains in the airspace and is used to determinethe fluid volume remaining in the isolated lung (3). The decreasein ²²Na⁺ and ³H-mannitol in the instillate is used to calculate the total andpassive small solute and fluid movement.

Experimental Protocols

In isolated lungs where drugs were added to the alveolar instillate, the compounds were present throughout the course of theexperiment. When substances were perfused through the pulmonaryvasculature, the compounds were added to the perfusate at thestart of the experiment and were present throughout the instillationprocedure, including the 10-min stabilization period. Dopamine(Sigma Chemical Co., St. Louis, MO) was freshly prepared beforeeach experiment as a 1,000× stock in normal saline. Amiloride(Sigma) was prepared as a 25 mM stock and added to the instillatefluid to obtain the final concentration used. Ouabain (ICN Biochemicals,Aurora, OH) was dissolved in 200 µl DMSO before addition to theperfusate.

A total of 78 isolated perfused rat lungs were studied. The experimental groups were as follows, with the number of animalsin each group in parentheses: controls (n = 12); dopamine administeredvia the airway instillate at concentrations of 10¹⁰ M (n = 6), 10⁹ M (n = 4), 10⁸ M (n = 6), 10⁶ M (n = 6), and 10⁴ M (n = 8); dopamine administered via the perfusate at concentrationsof 10⁸ M (n = 5), 10⁶ M (n = 6), and 10⁴ M (n = 4); treatment with amiloride via the airway instillateto inhibit epithelial apical sodium channels, using concentrationsof 10⁶ M amiloride (n = 4), 10⁶ M amiloride + 10⁴ M instilled dopamine (n = 5), 10⁴ M amiloride (n = 4), and 10⁴ M amiloride + 10⁴ M instilled dopamine (n = 5); and treatment with ouabain viathe perfusate to inhibit basolateral Na,K-ATPase, with concentrationsof 5 × 10⁴ M ouabain (n = 4) and 5 × 10⁴ M ouabain + 10⁴ M instilled dopamine (n = 3).

Calculations

The derivation of all equations involved in the mathematical model of edema clearance has been previously described in detail(3). Concentration of EBD-albumin was used to estimate airspacevolume. As virtually all EDB-albumin remains in the airspace,we may calculate instillate volume (V) at a given time t as:

Vt=V0[EBD]0/[EBD]t

where V₀ is the initial volume instilled and [EBD]₀ and [EBD]_t are the concentrations of EBD-albumin at times 0 and t, respectively.The removal of sodium from the alveolar space during a definedperiod of time is probably accompanied by isotonic water fluxand is given by:

JNa,
net=JNa,out−JNa,in

where J_Na,net is the net or active Na⁺ transport, J_Na,out is the total or unidirectional Na⁺ outflux and J_Na,in is the back flux of Na⁺ into the alveolar fluid by passive bidirectional movement. SinceNa⁺ concentration [Na⁺] remains constant in all compartments, the net Na⁺ flux (which we refer to as active Na⁺ transport) from the airspace is:

JNa,net=(V0−Vt)[Na+]/t

The unidirectional outflux of Na⁺ (J_Na,out) from the alveolar space, a result of active transport and passive movement, wascalculated as:

JNa,out=JNa,net {<FENCE>ln <FR><NU>[ Na22]t</NU><DE>[ Na22]0</DE></FR>/ln <FR><NU>Vt</NU><DE>V0</DE></FR></FENCE>+1}

Similarly, the (unidirectional) volume flux of ³H-mannitol (typically expressed as PA, permeability of surface area) was calculatedas:

PA=<FR><NU>(V0−Vt)</NU><DE>t</DE></FR><FENCE>ln <FR><NU>[ 3H-mannitol]t</NU><DE>[ 3H-mannitol]0</DE></FR>/ ln <FR><NU>Vt</NU><DE>V0</DE></FR></FENCE>

Albumin flux from the pulmonary circulation into the alveolar space was determined from the fraction of FITC-albumin thatappears in the alveolar space during the experimental protocol.For reasons of comparison fluxes are reported as volume fluxes(volume/time) by using the appropriate solute concentrations.

Measurement of cAMP

Levels of cAMP were measured in lung homogenates prepared following physiologic determinations in control lungs and lungsinstilled with 10⁶ M dopamine. Crude homogenates were passed over anion exchangecolumns (Amprep SAX; Amersham, Arlington Heights, IL) and theeluted cAMP preparations were lyophilized and redissolved in assaybuffer. Amounts of cAMP were determined by a commercial ELISA(Amersham) and were expressed as pg/lungs.

Statistical Analysis

All data are presented as mean ± SEM. Analysis of variance was used to test for differences between groups, followed by amultiple comparisons test (Tukey) when the F statistic indicatedsignificance.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

In isolated perfused lungs, instilled dopamine increased lung liquid clearance (Figure 1) out of the alveoli. The increasedclearance was dose-dependent, with 10⁸ M and greater concentrations of dopamine increasing clearanceto 27 to 33% above controls (p < 0.05). Dopamine at any of theconcentrations utilized did not affect passive sodium or manitolflux (Table 1, p = 0.75 for Na⁺, p = 0.93 for mannitol) or increase epithelial permeability,as monitored by FITC-albumin flux (Table 2). Perfusate flow didnot change with the administration of dopamine (Table 2). Inmost experiments, dopamine was placed in the instillate to maximizethe concentration at the epithelial cell level. When added tothe perfusate, dopamine increased clearance although the effectwas not consistent at 10⁶ M (Figure 2).

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Figure 1. Dose-response of increased lung liquid clearance in response to increasing concentrations of dopamine in the isolated perfusedlung. Dopamine at the indicated concentrations was added to theinstillate. *p < 0.05 as compared with controls.

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TABLE 1

PASSIVE SODIUM AND MANNITOL FLUXES IN ISOLATED PERFUSED RAT LUNGS^*

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TABLE 2

PERFUSATE FLOWS AND ALBUMIN FLUXES IN ISOLATED PERFUSED RAT LUNGS^*

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Figure 2. Dose-response of increased lung liquid clearance seen when dopamine was perfused through the pulmonary circulation at theindicated concentrations. *p < 0.05 as compared with controls.

To determine the cellular pathway for sodium transport affected by dopamine, we used both amiloride to block sodium channelsand ouabain to specifically block Na,K-ATPase in the absence andpresence of dopamine.

Two different doses of amiloride were used in our studies. As shown in Figure 3, amiloride inhibited active sodium transportand lung liquid clearance. When lungs were instilled with 10⁶ M amiloride, clearance decreased to 66% of control values, while10⁴ M amiloride decreased clearance to 51% of controls. When amiloridewas coinstilled with 10⁴ M dopamine, 10⁴ M amiloride completely inhibited the dopamine-stimulated clearance(89% of 10⁴ M amiloride alone), while dopamine was still able to elicit anincrease in clearance when coinstilled with 10⁶ M amiloride (154% of 10⁶ M amiloride alone). Passive sodium and mannitol flux were notaffected by either dose of amiloride in the presence or absenceof dopamine (Table 1, p = 0.47 for Na⁺, p = 0.78 for mannitol); permeability to albumin was also notchanged (Table 2). Perfusate flow was not significantly differentin any group (Table 2).

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Figure 3. Amiloride instilled into the alveolar space inhibited alveolar liquid clearance. The effect of amiloride on dopamine-stimulatedclearance was dependent upon the dose of amiloride used. Dopamineconcentration was 10⁴ M. Amil: Amiloride at the indicated concentrations. *p < 0.05as compared with control. ⁺p < 0.05 as compared with low amiloride alone or with high amilorideplus dopamine. There was no significant difference from dopaminealone.

We then determined whether ouabain, the specific inhibitor of Na,K-ATPase, inhibited sodium transport and lung liquid clearance(Figure 4). Ouabain (5 × 10⁴ M) decreased clearance to 45% of controls, and also eliminatedthe stimulation of clearance by dopamine (ouabain with 10⁴ M dopamine was 86% of ouabain alone). Passive sodium and mannitolfluxes (Table 1, p = 0.46 for Na⁺, p = 0.67 for mannitol) and albumin flux (Table 2) were notsignificantly different. Perfusate flow was not different (Table2).

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Figure 4. Ouabain (5 × 10⁴ M) perfused through the pulmonary circulation inhibited lung liquid clearance in both control lungs and inlungs instilled with 10⁴ M dopamine. *p < 0.05 as compared with controls. +p < 0.05 comparedwith dopamine alone. Dopamine did not increase clearance in ouabain-perfusedlungs.

Cyclic AMP measurements were performed in lung homogenates from controls (n = 5) and from lungs instilled with 10⁶ M dopamine (n = 4). The amount of cAMP calculated per set oflungs did not increase significantly following incubation withdopamine (30.7 ± 15.6 pmol versus 25.8 ± 6.1 pmol for controllungs).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Regulation of sodium transport and consequently edema clearance by the alveolar epithelium might potentially provide new approachesto clinical management of patients with pulmonary edema. In thepresent studies we have demonstrated that dopamine, which is alreadywidely used clinically, stimulates clearance of alveolar edemain the isolated perfused rat lung in a dose-dependent manner (Figures1 and 2). We evaluated mechanisms contributing to the increasedlung liquid clearance by selectively inhibiting components ofthe sodium pathway in the cell, using both amiloride and ouabain,inhibitors of sodium channels and Na,K-ATPase, respectively. Wefocused on the mechanisms that contribute significantly to vectorialsodium flux, although we recognize that other mechanisms outsidethe scope of this manuscript (Na-glucose exchange and Na-H exchange,for example) could also contribute to transpulmonary sodium flux(14).

Because $beta$ -adrenergic agonists, another class of catecholamines, stimulate clearance and increase the activity of epithelialsodium channels (16, 18, 19), we instilled lungs with amilorideto inhibit the sodium channels (Figure 3). At 10⁶ M, which specifically inhibits sodium channels, the stimulatoryeffect of dopamine on clearance was preserved, albeit at a lowertotal clearance. At 10⁴ M amiloride, the ability of dopamine to stimulate sodium transportand liquid clearance was fully inhibited. As amiloride at higherconcentrations is known to inhibit several sodium transport mechanismsin addition to sodium channels, including Na,K-ATPase (20),we hypothesized that when the residual stimulatory effect of dopamineseen in the presence of 10⁶ M amiloride was abolished by 10⁴ M amiloride, we could be inhibiting the sodium pump as well.Even if the sodium channels are not 100% inhibited (and we agreethat at 10⁶ M, they are probably not), the proportion of fluid transportthat is amiloride-sensitive should increase if an increase insodium channel activity is necessary to increase overall clearance.We did not see an increase in this proportion, leading us to concludethat the increased clearance produced by dopamine was probablynot mediated by an increase in sodium channel activity, but ratherby other mechanisms.

We then perfused lungs with 5 × 10⁴ M ouabain to specifically inhibit Na,K-ATPase. In these lungs, however, not only was basalliquid clearance decreased, the dopamine-stimulated increasedin lung fluid clearance was abolished (Figure 4). These data suggestthat dopamine increases lung liquid clearance by stimulating activeNa⁺ transport. Although this study does not allow us to deduce theexact mechanism responsible for the increase in Na⁺ transport, the time course of this stimulation suggests a short-termregulation of the transport mechanisms (for example, translocationor recruitment of new Na⁺ pumps to the cell membrane), because it is unlikely that synthesisof new Na,K-ATPase protein occurred within the time frame involved.

Most of the previous work concerning regulation of Na,K-ATPase by dopamine and the mechanisms of regulation (second messengersystems, protein phosphorylation, cytoskeletal effects, etc.)has concentrated on the transporting epithelial cells of the kidneyand dopamine-sensitive cells of the central nervous system (21,22). While these studies define the short-term regulation ofNa,K-ATPase in the tissues mentioned, the behavior of other celltypes may very well be different, as pump regulation is likelydetermined by the different functions of the cells. For example,in the small intestine, which shares its embryological originswith the lungs, dopamine has been found to stimulate sodium absorption(23), while in renal tubules, the effects of dopamine on sodiumtransport are generally inhibitory (7, 22). Clearly, evenwithin different types of epithelial cells regulation of Na,K-ATPasemay vary from one cell type to another.

We are not aware of any previous publications on the effect of dopamine as a possible short-term modulator of lung Na,K-ATPaseactivity and lung liquid clearance. Recently, an abstract waspresented in a different model in which dobutamine, but not dopamine,increased lung edema clearance (24); other laboratories havebegun to explore the possible cellular mechanisms of sodium transportor lung edema clearance by other mediators.

Regulation of Na,K-ATPase activity and consequently sodium movement in transporting epithelia may have important physiologicconsequences. Regulation of Na,K-ATPase varies in different organsand cell lines (6, 25), with evidence that mechanisms mediatedby cAMP-dependent protein kinase (PKA) or protein kinase C (PKC)may play important intracellular signaling roles. Activation ofthese cellular pathways has also been shown to affect other transportersinvolved in cellular sodium homeostasis, notably the activationof sodium channels by cAMP (19, 29). Although the mechanismof regulation cannot be deduced from the current study, it hasprovided us with a model of short-term sodium transport and edemaclearance upregulation to study in the alveolar epithelium.

It has been demonstrated by several groups of investigators that administration of cyclic AMP analogues (30) or agents thatincrease intracellular cAMP (15, 17, 30, 31) increasesbasal lung liquid clearance and sodium transport across the alveolarepithelium. It has also been shown that this is likely an importantphysiological means of regulating these processes, as shown byincreased catecholamine release, which mediates enhanced lungliquid clearance in septic shock (16), and by the finding thatincreased intracellular cAMP can stimulate edema clearance followingischemia-reperfusion lung injury (32). The effects of dopamine,however, appear to be distinct from those of $beta$ -adrenergic agonists,as isoproterenol or terbutaline have been reported to produceclearances which are approximately twice controls (31, 33,34), and are greater than the increase we saw with dopamine(33%).

In many cell types, dopamine activates cAMP via D₁ (or DA₁) type dopamine receptors (7, 21, 22). We therefore postulatedthat the effects of dopamine in our isolated perfused lung modelcould have been mediated through this pathway. Our findings werenot definitive, as we were able to measure only a small (nonsignificant)increase in cAMP levels in lung homogenates following incubationwith dopamine. These data agree with studies in renal corticalplasma membranes in which D₁ receptor occupation activated signaltransduction pathways independent of cAMP (35). Unfortunately,we cannot rule out the possibility that there was an increasein cAMP which we were unable to detect, either because of dilutionof epithelial cAMP by other cells present in lung tissue, or bya degradation of any initial increase in cAMP over the courseof the experiment. Further experiments at the cellular level willbe necessary to more definitively resolve both which receptortype is activated and which second messenger system is responsiblefor the observed increase in clearance.

In summary, our data show that dopamine stimulates lung liquid clearance in a dose-dependent manner. As this stimulation isinhibited by ouabain or amiloride, it is likely that dopamineexerts its effects by increasing active Na⁺ transport. Furthermore, the ability of ouabain but not low concentrationsof amiloride to inhibit the dopamine-stimulated Na⁺ transport and lung liquid clearance, leads us to reason thatthis occurs via a modulation of the lung Na,K-ATPase. While itis beyond the scope of this manuscript to comment on the cellularpathways which are involved in mediating the response to dopamine,further studies are warranted to define the cellular mechanismsin detail.

	Footnotes

Correspondence and requests for reprints should be addressed to Jacob I. Sznajder, M.D., Columbia Michael Reese Hospital and Medical Center, Pulmonary Research Laboratory, 2929 S. Ellis, RC-216, Chicago, IL 60616.

(Received in original form October 4, 1996 and in revised form April 23, 1997).

This research was supported in part by grants from the American Heart Association 96012890, NIH HL48129, and funds providedby the Department of Medicine, Columbia Michael Reese Hospital.J.I.S. is a Career Investigator of the American Lung Association.

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E. Lecuona, L. A. Dada, H. Sun, M. L. Butti, G. Zhou, T.-L. Chew, and J. I. Sznajder
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FASEB J, December 1, 2006; 20(14): 2618 - 2620.
[Abstract] [Full Text] [PDF]

Z. S. Azzam, Y. Adir, L. Welch, J. Chen, J. Winaver, P. Factor, N. Krivoy, A. Hoffman, J. I. Sznajder, and Z. Abassi
Alveolar fluid reabsorption is increased in rats with compensated heart failure
Am J Physiol Lung Cell Mol Physiol, November 1, 2006; 291(5): L1094 - L1100.
[Abstract] [Full Text] [PDF]

M. N. Helms, J. Self, H. F. Bao, L. C. Job, L. Jain, and D. C. Eaton
Dopamine activates amiloride-sensitive sodium channels in alveolar type I cells in lung slice preparations
Am J Physiol Lung Cell Mol Physiol, October 1, 2006; 291(4): L610 - L618.
[Abstract] [Full Text] [PDF]

H. G. Folkesson and M. A. Matthay
Alveolar Epithelial Ion and Fluid Transport: Recent Progress
Am. J. Respir. Cell Mol. Biol., July 1, 2006; 35(1): 10 - 19.
[Full Text] [PDF]

M. N. Helms, X.-J. Chen, S. Ramosevac, D. C. Eaton, and L. Jain
Dopamine regulation of amiloride-sensitive sodium channels in lung cells
Am J Physiol Lung Cell Mol Physiol, April 1, 2006; 290(4): L710 - L722.
[Abstract] [Full Text] [PDF]

R. Jain and A. DalNogare
Pharmacological Therapy for Acute Respiratory Distress Syndrome
Mayo Clin. Proc., February 1, 2006; 81(2): 205 - 212.
[Abstract] [Full Text] [PDF]

A. M. Bertorello and J. I. Sznajder
The Dopamine Paradox in Lung and Kidney Epithelia: Sharing the Same Target but Operating Different Signaling Networks
Am. J. Respir. Cell Mol. Biol., November 1, 2005; 33(5): 432 - 437.
[Abstract] [Full Text] [PDF]

G. M. Mutlu and J. I. Sznajder
Mechanisms of pulmonary edema clearance
Am J Physiol Lung Cell Mol Physiol, November 1, 2005; 289(5): L685 - L695.
[Abstract] [Full Text] [PDF]

Z. S. Azzam, Y. Adir, A. Crespo, A. Comellas, E. Lecuona, L. A. Dada, N. Krivoy, D. H. Rutschman, J. I. Sznajder, and K. M. Ridge
Norepinephrine Increases Alveolar Fluid Reabsorption and Na,K-ATPase Activity
Am. J. Respir. Crit. Care Med., October 1, 2004; 170(7): 730 - 736.
[Abstract] [Full Text] [PDF]

Y. Adir, Z. S. Azzam, E. Lecuona, S. Leal, L. Pesce, V. Dumasius, A. M. Bertorello, P. Factor, J. B. Young, K. M. Ridge, et al.
Augmentation of Endogenous Dopamine Production Increases Lung Liquid Clearance
Am. J. Respir. Crit. Care Med., March 15, 2004; 169(6): 757 - 763.
[Abstract] [Full Text] [PDF]

Y. Adir, P. Factor, V. Dumasius, K. M. Ridge, and J. I. Sznajder
Na,K-ATPase Gene Transfer Increases Liquid Clearance during Ventilation-induced Lung Injury
Am. J. Respir. Crit. Care Med., December 15, 2003; 168(12): 1445 - 1448.
[Abstract] [Full Text] [PDF]

A. P. Comellas, L. M. Pesce, Z. Azzam, F. J. Saldias, and J. I. Sznajder
Scorpion Venom Decreases Lung Liquid Clearance in Rats
Am. J. Respir. Crit. Care Med., April 15, 2003; 167(8): 1064 - 1067.
[Abstract] [Full Text] [PDF]

C. Sartori and M.A. Matthay
Alveolar epithelial fluid transport in acute lung injury: new insights
Eur. Respir. J., November 1, 2002; 20(5): 1299 - 1313.
[Abstract] [Full Text] [PDF]

L. B. Ware, X. Fang, Y. Wang, T. Sakuma, T. S. Hall, and M. A. Matthay
Lung Edema Clearance: 20 Years of Progress: Selected Contribution: Mechanisms that may stimulate the resolution of alveolar edema in the transplanted human lung
J Appl Physiol, November 1, 2002; 93(5): 1869 - 1874.
[Abstract] [Full Text] [PDF]

J. L. Fisher and S. S. Margulies
Na+-K+-ATPase activity in alveolar epithelial cells increases with cyclic stretch
Am J Physiol Lung Cell Mol Physiol, October 1, 2002; 283(4): L737 - L746.
[Abstract] [Full Text] [PDF]

M. A. Matthay, H. G. Folkesson, and C. Clerici
Lung Epithelial Fluid Transport and the Resolution of Pulmonary Edema
Physiol Rev, July 1, 2002; 82(3): 569 - 600.
[Abstract] [Full Text] [PDF]

F. J. Saldias, A. P. Comellas, L. Pesce, E. Lecuona, and J. I. Sznajder
Dopamine increases lung liquid clearance during mechanical ventilation
Am J Physiol Lung Cell Mol Physiol, July 1, 2002; 283(1): L136 - L143.
[Abstract] [Full Text] [PDF]

R. G. Brower, L. B. Ware, Y. Berthiaume, and M. A. Matthay
Treatment of ARDS
Chest, October 1, 2001; 120(4): 1347 - 1367.
[Abstract] [Full Text] [PDF]

C. Guerrero, E. Lecuona, L. Pesce, K. M. Ridge, and J. I. Sznajder
Dopamine regulates Na-K-ATPase in alveolar epithelial cells via MAPK-ERK-dependent mechanisms
Am J Physiol Lung Cell Mol Physiol, July 1, 2001; 281(1): L79 - L85.
[Abstract] [Full Text] [PDF]

L. B. WARE and M. A. MATTHAY
Alveolar Fluid Clearance Is Impaired in the Majority of Patients with Acute Lung Injury and the Acute Respiratory Distress Syndrome
Am. J. Respir. Crit. Care Med., May 1, 2001; 163(6): 1376 - 1383.
[Abstract] [Full Text]

Z. S. Azzam, F. J. Saldias, A. Comellas, K. M. Ridge, D. H. Rutschman, and J. I. Sznajder
Catecholamines increase lung edema clearance in rats with increased left atrial pressure
J Appl Physiol, March 1, 2001; 90(3): 1088 - 1094.
[Abstract] [Full Text] [PDF]

J. A. Frank, Y. Wang, O. Osorio, and M. A. Matthay
beta -Adrenergic agonist therapy accelerates the resolution of hydrostatic pulmonary edema in sheep and rats
J Appl Physiol, October 1, 2000; 89(4): 1255 - 1265.
[Abstract] [Full Text] [PDF]

A. G. Therien and R. Blostein
Mechanisms of sodium pump regulation
Am J Physiol Cell Physiol, September 1, 2000; 279(3): C541 - C566.
[Abstract] [Full Text] [PDF]

G. M. Verghese, L. B. Ware, B. A. Matthay, and M. A. Matthay
Alveolar epithelial fluid transport and the resolution of clinically severe hydrostatic pulmonary edema
J Appl Physiol, October 1, 1999; 87(4): 1301 - 1312.
[Abstract] [Full Text] [PDF]

M. L. BARNARD, K. M. RIDGE, F. SALDIAS, E. FRIEDMAN, M. GARE, C. GUERRERO, E. LECUONA, A. M. BERTORELLO, A. I. KATZ, and J. I. SZNAJDER
Stimulation of the Dopamine 1 Receptor Increases Lung Edema Clearance
Am. J. Respir. Crit. Care Med., September 1, 1999; 160(3): 982 - 986.
[Abstract] [Full Text]