Protease Modulation of the Activity of the Epithelial Sodium Channel Expressed in Xenopus Oocytes

doi:10.1085/jgp.111.1.127

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Protease Modulation of the Activity of the Epithelial Sodium Channel Expressed in Xenopus Oocytes

Ahmed Chraïbi, Véronique Vallet, Dmitri Firsov, Solange Kharoubi Hess, and Jean-Daniel Horisberger

From the Institute of Pharmacology and Toxicology, University of Lausanne, CH-1005 Lausanne, Switzerland

ABSTRACT

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We have investigated the effect of extracellular proteases onthe amiloride-sensitive Na⁺ current (I_Na) in Xenopus oocytesexpressing the three subunits ${alpha}$ , β, and ${gamma}$ of the rat or Xenopusepithelial Na⁺ channel (ENaC). Low concentrations of trypsin(2 µg/ml) induced a large increase of I_Na within a fewminutes, an effect that was fully prevented by soybean trypsininhibitor, but not by amiloride. A similar effect was observedwith chymotrypsin, but not with kallikrein. The trypsin-inducedincrease of I_Na was observed with Xenopus and rat ENaC, andwas very large ( $~$ 20-fold) with the channel obtained by coexpressionof the ${alpha}$ subunit of Xenopus ENaC with the β and ${gamma}$ subunitsof rat ENaC. The effect of trypsin was selective for ENaC, asshown by the absence of effect on the current due to expressionof the K⁺ channel ROMK2. The effect of trypsin was not preventedby intracellular injection of EGTA nor by pretreatment withGTP- ${gamma}$ S, suggesting that this effect was not mediated by G proteins. Measurement of the channel protein expression at the oocytesurface by antibody binding to a FLAG epitope showed that theeffect of trypsin was not accompanied by an increase in thechannel protein density, indicating that proteolysis modifiedthe activity of the channel present at the oocyte surface ratherthan the cell surface expression. At the single channel level,in the cell-attached mode, more active channels were observedin the patch when trypsin was present in the pipette, whileno change in channel activity could be detected when trypsinwas added to the bath solution around the patch pipette. Weconclude that extracellular proteases are able to increase the open probability of the epithelial sodium channel by aneffect that does not occur through activation of a G protein-coupledreceptor, but rather through proteolysis of a protein that iseither a constitutive part of the channel itself or closelyassociated with it.

Key Words: trypsin • chymotrypsin • amiloride • G protein • epithelial Na⁺ channel

Address correspondence to Jean-Daniel Horisberger, Instituteof Pharmacology and Toxicology, University of Lausanne, Bugnon27, CH-1005 Lausanne, Switzerland. Fax: 41 21 692 53 55; E-mail:jean-daniel.horisberger{at}ipharm.unil.ch

introduction

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The passage of sodium through the epithelial Na⁺ channel (ENaC)¹is the rate limiting step in the sodium reabsorption by theepithelial cells of the distal nephron and colon and in airways(Garty and Palmer, 1997). It thereby plays a key role in theregulation of the sodium balance, extracellular fluid volume,and blood pressure by the kidney, and in the controlled fluidreabsorption in the airways. The activity of ENaC has to betightly regulated with regard to the whole organism sodiumbalance, but also with regards to the epithelial cell transportcapacity so that the homeostasis of the intracellular milieuis preserved. This regulation is under the control of severalhormones and intracellular factors by mechanisms that are notyet completely understood (Garty and Palmer, 1997).

Concerning luminal factors, Garty and Edelman (1983) observedthat trypsin, at a concentration of 1 mg/ml, induced an irreversibleinhibition of the sodium transport and this effect could beprevented by amiloride. They concluded that a component ofthe Na⁺ channel protein could be cleaved by a protease at a site protectable by amiloride bound to its receptor. Lewisand Alles (1986) and Lewis and Clausen (1991) studied the effectsof proteases such as kallikrein, which is normally presentin mammalian urine, on the Na⁺ channel of the rabbit urinarybladder. To briefly summarize their findings, they observedthat these proteases altered the highly selective and amiloride-sensitiveNa⁺ channel into a nonselective cation channel, and furtherproteolysis rendered this channel unstable in the membraneso that the proteolyzed channel could eventually be recoveredfrom the fluid bathing the apical medium (Zweifach and Lewis,1988). These authors speculated that luminal proteolytic activity could be a physiological regulator of the epithelial Na⁺ channel(Lewis and Alles, 1986).

Orce et al. (1980) made an interesting observation suggesting,in contrast, that an extracellular protease was able to activatethe electrogenic Na⁺ transport: they reported that the trypsininhibitor aprotinin induced a decrease of the amiloride-sensitiveshort circuit current in the toad bladder. In support of anactivating effect of a protease on ENaC, Vallet et al. (1997)have recently identified a novel endogenous serine protease in A6 cells that is able to activate the amiloride-sensitive Na⁺ current when coexpressed with ENaC in oocytes. In addition,they also show that trypsin can activate the amiloride-sensitiveNa⁺ current in the A6 cell. To try to understand the mechanismof these effects of proteases, we have studied the effect ofserine proteases on the Na⁺ current carried by rat (Canessaet al., 1993, 1994) or Xenopus (Puoti et al., 1995) ENaC expressed in Xenopus oocytes. Trypsin is known to induce a transientactivation of a calcium-activated chloride current in Xenopusoocytes, an effect described by Durieux et al. (1994) thatis mediated through a G protein-coupled trypsin receptor naturallypresent in the oocyte membrane and an IP3-induced release ofcalcium from intracellular stores. In addition to these knowneffects, we observed that low concentrations of trypsin orchymo-trypsin induced an activation of the amiloride-sensitive current carried by ENaC expressed in oocytes. A number of experimentsperformed to evaluate the role of G proteins or potential intracellularsecond messengers in this regulation yielded negative results.The data from macroscopic current and single channel experimentsrather suggest that the effect of trypsin occurs through proteolysisof the channel protein itself or of a closely associated protein.

methods

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Expression of Rat and Xenopus ENaC in Xenopus Oocytes
In vitro-transcribed cRNA for the ${alpha}$ , β, and ${gamma}$ subunits ofXenopus ENaC (XENaC) and rat ENaC (rENaC) were injected intostage V–VI Xenopus oocytes (0.3–1 ng of cRNA ofeach subunit in a total volume of 50 nl) as described previously(Canessa et al., 1993, 1994; Puoti et al., 1995). Electrophysiologicalexperiments were performed 1–2 d after cRNA injection.In other experiments, 1 ng of human cystic fibrosis transmembraneconductance regulator (CFTR) cRNA (clone generously providedby R. Boucher, University of North Carolina, Chapel Hill, NC),1 ng of human β2 adrenergic receptor cRNA (clone generouslyprovided by S. Cotecchia, Institute of Pharmacology, Lausanne,Switzerland), or 0.1 ng rat ROMK2 cRNA (cDNA generously providedby L.G. Palmer, Cornell University Medical College, New York)were in vitro transcribed and injected into Xenopus oocytes.

Ion Current Measurement in Whole Ooctyes
Amiloride-sensitive and cAMP-stimulated Cl^– currents weremeasured as previously described (Canessa et al., 1993) usingthe two-electrode voltage clamp technique by means of a DaganTEV voltage clamp apparatus (Dagan Corp., Minneapolis, MN),at room temperature (22–25°C) and at a holding potentialof –100 mV in a solution containing (mM) 100 Na gluconate,0.4 CaCl₂, 10 Na HEPES, pH 7.4, 5 BaCl₂, and 10 tetraethylammoniumchloride. The current signal was filtered at 20 Hz using theinternal filter of the Dagan apparatus and continuously recordedon a paper chart. Low chloride concentration and K⁺ channelblockers were used to reduce the background membrane conductance.

ROMK2-induced K⁺ currents were measured as the inward currentinduced by addition of 5 mM K⁺ at –100 mV under the conditionsdescribed by Zhou et al. (1994).

Single Channel Recordings
Before patch-clamp experiments, the oocytes were placed for3–5 min at room temperature in a hypertonic medium (475mosM) with the following composition (mM): 200 K aspartate,20 KCl, 1 MgCl₂, 10 EGTA, 10 Na HEPES, pH 7.4. The vitellinemembrane could then be manually removed from the cell usingfine forceps (Methfessel et al., 1986). The oocytes were thenimmediately transferred to the recording chamber.

Both the cell-attached and excised outside-out patch clamp experimentswere carried out according to the methods described by Hamillet al. (1981). Patch pipettes were made of borosilicate glass(Corning Glass Works, Corning, NY), pulled in two stages witha PP-83 vertical puller (Narishige, Japan) and fire polished. They had a resistance of 10–20 M ${Omega}$ . Single channel currentswere recorded with a patch clamp amplifier (LM EPC 7; ListElectronics, Darmstadt, Germany), displayed on an oscilloscope(Tektronix, Heerenveen, The Netherlands) and stored on a digital tape recorder (Biologic, France). By convention, for outside-out patches the intracellular potential corresponds to the pipettepotential (V_pip), and negative (downward) single channel currents correspond to Li⁺ flux from the extracellular to the intracellular side of the membrane; for cell-attached patches the membrane potential should be close to the actual potential across themembrane patch because the oocyte membrane potential is closeto 0 mV under our experimental conditions.

Current signals were filtered at 200 Hz with an eight pole Bessel filter (Frequency Devices Inc., Haverhill, MA) and digitizedat 1 kHz using a Labmaster analog–digital interface and Fetchex Software (Axon Instruments, Foster City, CA). The n.Po product (n = number of channel, Po = open probability) was calculated as n.Po = I_ENaC/i, where I_ENaC is the current dueto ENaC (= total current minus current with no channel open)averaged over a 1-min recording, divided by the unitary current measured as the peak to peak interval in the amplitude histogram.

Chemicals and Enzymes
Amiloride, guanosine 5'-O-(3-thiotriphosphate) (GTP- ${gamma}$ S), soybeantrypsin inhibitor, and trypsin (DPCC-treated trypsin from bovinepancreas, a form of trypsin with low level of chymotrypsin contamination) were obtained from Sigma Chemical Co. (St. Louis,MO). Porcine kallikrein was obtained from Calbiochem Corp.(La Jolla, CA) and chymotrypsin (TLCK-treated ${alpha}$ -chymo-trypsin,a form of chymotrypsin with a low level of trypsin contamination),was purchased from Fluka (Buchs, Switzerland).

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Effect of Trypsin on ENaC Expressed in Xenopus Oocytes
As shown in Fig. 1 a, 2 µg/ml trypsin had a biphasic effect:it induced first a peak of inward current lasting 10–60s; the amplitude and the duration of this current was highlyvariable, sometimes undetectable and sometimes amounting to2–3 µA. This effect of trypsin has been describedby Durieux et al. (1994). This current could also be observedin native noninjected oocytes or oocytes expressing ENaC inthe presence of 10 µM amiloride and was therefore notrelated to ENaC. In oocytes expressing ${alpha}$ β ${gamma}$ ENaC, trypsininduced in addition a slower increase of a steady inward current,with a time course of 1–5 min to reach its maximal amplitude (Fig. 1 a). This current was amiloride sensitive.

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Figure 1 Effect of trypsin on the amiloride-sensitive current in oocytes expressing ${alpha}$ β ${gamma}$ ENaC. (a) Original current recording in an oocyte expressing ${alpha}$ β ${gamma}$ rENaC. The current sensitive to 10 µM amiloride was measured at –100 mV before and after a 4-min exposure to 2 µg/ml trypsin. A transient spike of current, attributed to Ca-activated Cl channels occurs in the 10–20 s after the beginning of trypsin treatment, and there is an approximately threefold increase in the amiloride-sensitive current. (b) Original current recording in an oocyte expressing ${alpha}$ β ${gamma}$ XENaC. The current sensitive to 10 µM amiloride was measured at –100 mV before and after 4-min exposures to 2 µg/ml trypsin, first in the presence of 10 µg/ml soybean trypsin inhibitor, and then without inhibitor. Trypsin has no detectable effect on either I_Na or a chloride current in the presence of the inhibitor. (c) Original current recording in an oocyte expressing ${alpha}$ β ${gamma}$ rENaC. The current sensitive to 10 µM amiloride was measured at –100 mV before and after a 4-min exposure to 2 µg/ml trypsin in the presence of 10 µM amiloride. A transient increase in current, corresponding to the Ca-activated Cl^– current can be observed $~$ 1 min after the beginning of exposure to trypsin. A more than twofold increase is seen when amiloride is removed after trypsin treatment.

The amplitude of the increase of the amiloride-sensitive sodiumcurrent (I_Na) was quite variable, ranging from a hardly detectableincrease to a sixfold increase in oocytes expressing rat ${alpha}$ β ${gamma}$ ENaC,and a 2- to more than 10-fold increase in oocytes expressingXenopus ${alpha}$ β ${gamma}$ ENaC. Heteromeric channels composed of the ${alpha}$ subunit of the Xenopus ENaC and the β and ${gamma}$ subunits ofrat ENaC expressed a small I_Na, but in these oocytes trypsininduced a very large increase of I_Na, often >20-fold, followingthe same time course. The mean values of the baseline I_Na andof the increase of I_Na after a 3–5-min exposure to 2 µg/mltrypsin in Xenopus ENaC, ( ${alpha}$ XβX ${gamma}$ X), in rat ENaC ( ${alpha}$ rβr ${gamma}$ r),and in heteromeric rat/Xenopus channels, ${alpha}$ Xβr ${gamma}$ r and ${alpha}$ rβX ${gamma}$ X,are given in Table I. The response to trypsin was inverselycorrelated with the initial I_Na value as shown in Fig. 2, suggestingthat trypsin effect was larger in oocytes either expressinga low number of channels or channels with a low open probability.

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Table I Effect of Trypsin on the Amiloride-sensitive Na⁺ Current (I_Na)

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Figure 2 Trypsin-induced increase in amiloride-sensitive Na current (I_Na): relationship to the initial I_Na value. The increase in I_Na after a 3–5-min exposure to 2 µg/ml trypsin is reported as a function of the initial value of I_Na in 31 oocytes expressing ${alpha}$ β ${gamma}$ Xenopus ENaC. Note that both scales are logarithmic. The straight line is the regression line of log(increase in I_Na) versus log(I_Na). The corresponding r = 0.5794 (n = 31), indicating a statistically significant inverse relationship (P < 0.001) between these two variables.

To examine the question of whether the effect of trypsin wasdue to its catalytic activity or to some other mechanism suchas binding to a receptor, we measured the effect of trypsin(2 µg/ml) first in the presence and then absence of fivefoldexcess of soybean trypsin inhibitor (10 µg/ml) in oocytesexpressing ${alpha}$ β ${gamma}$ rENaC. As shown in the example of Fig. 1 b,the presence of trypsin inhibitor completely prevented theeffect of trypsin, while trypsin alone was subsequently ableto induce a large increase of I_Na. In eight measurements, a 3-min exposure to trypsin + trypsin inhibitor resulted ina slight decrease of I_Na to 87 ± 13% of its initial value (no significant difference), while subsequent exposure totrypsin alone induced an increase of I_Na to 277 ± 36%of the initial control value (P < 0.001, paired t test).

The inhibitory effect of trypsin described earlier in toador rabbit bladder (Garty and Edelman, 1983; Lewis and Clausen,1991) could be prevented by amiloride. We tested the effectof amiloride on the stimulatory effect of trypsin using thefollowing protocol to ensure that no channels were exposed totrypsin in the absence of amiloride (see example in Fig. 1c). After recording the Na⁺ current in the control solution,amiloride (10 µM) was first added to block the channel.30 s later, trypsin (2 µg/ml) was added in the presenceof amiloride for 3 min, and then removed while amiloride wasstill present. Finally, amiloride was removed, allowing measurementof the Na⁺ current. As shown in Fig. 1 c, the stimulatory effecton I_Na was not prevented by amiloride. In a series of comparativemeasurements, the increase of the amiloride-sensitive currentwhen trypsin was added for 3 min in the absence of amiloride(8.6 ± 1.6, n = 11) and when trypsin was added in thepresence of 10 µM amiloride (9.8 ± 2.1, n = 9)was similar.

To evaluate the selectivity of the action of trypsin, we alsostudied the effect of trypsin on the inward K⁺ current inducedin oocyte by expression of ROMK2, a renal K⁺ channel that ismost probably expressed in the apical membrane of the corticalcollecting tubule principal cells, the same membrane in whichENaC is expressed (Zhou et al., 1994). In 11 oocytes expressing ROMK2, the inward K⁺ current amounted to 365 ± 69 nAand was not increased by trypsin (331 ± 66 nA, after a 3-min exposure to 2 µg/ml trypsin).

Trypsin Concentration–Effect Relationship and Effects of Other Proteolytic Enzymes
Because of the large variability of the response to trypsinand the large and variable Cl^– current induced earlyafter exposure to trypsin, we were not able to establish a relationshipbetween the concentration of trypsin and the initial rate ofNa⁺ current increase. However, to demonstrate that a maximaleffect could be obtained by a 3-min exposure to a 2-µg/mltrypsin concentration, we showed that a subsequent 3-min exposureto 50 µg/ml trypsin could not further increase I_Na (seeFig. 3 a). In addition, in an attempt to observe the inhibitoryeffect described earlier, we measured I_Na in oocytes expressingENaC before and after a 3-min exposure to 10 µg/ml trypsin,a maneuver that induced the usual increase in I_Na, and thenwe incubated these oocytes for 30 min in a solution containing1 mg/ ml trypsin and measured I_Na again in the same oocytes. This experiment was performed in 18 oocytes expressing XenopusENaC and 14 oocytes expressing rat ENaC. In both cases, wefailed to observe a decrease of the Na⁺ current (Fig. 3 b).

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Figure 3 Response to high concentration of trypsin. The amiloride-sensitive current (I_Na) was measured before exposure to trypsin, first after a 3-min exposure to a 2-µg/ml concentration of trypsin, and then after a 3-min exposure to 50 µg/ml trypsin. Although the low concentration induced a significant increase of I_Na (P < 005, n = 8, paired student's t test), there was no significant further increase nor decrease of I_Na after the high concentration of trypsin. The amiloride-sensitive current (I_Na) was measured before exposure to trypsin, first after a 3-min exposure to a 2 µg/ml concentration of trypsin, and then after a 30-min incubation in a 1 mg/ml-containing bath solution (experimental group, filled symbols) or in the same solution without trypsin (control group, open symbols). Results are shown for oocytes expressing Xenopus ENaC (circles; experimental, n = 18; control, n = 8) and rat ENaC (open squares; experimental, n = 14; control, n = 12). In all groups, the first treatment with trypsin induced a significant increase of I_Na(P < 0.01 in each case). However, the long exposure to the high concentration of trypsin did not induce any significant further increase or decrease of I_Na. In the XENaC control group only, there was a small decrease (P < 0.02) of I_Na after the 30-min incubation in the control medium.

The effect of chymotrypsin on I_Na was roughly similar to theeffect of trypsin. With oocytes expressing Xenopus ${alpha}$ β ${gamma}$ ENaC,a 3-min treatment with 2 or 10 µg/ml induced a mean increaseof 1.50 ± 0.08-fold (n = 14) and 2.65 ± 0.36-fold(n = 13), respectively. With rat ENaC, 2 µg/ml chymotrypsininduced a 2.69 ± 0.33-fold increase in I_Na (n = 13).Remarkably, chymotrypsin never induced the early transientpeak of current that was usually observed with trypsin andattributed to a calcium-activated chloride channel.

We also tested the effect of kallikrein on oocytes expressingXenopus ENaC. Kallikrein, at a concentration of 10 µg/mland for a 5-min exposure, produced no detectable effect. Infact, I_Na decrease from 5.9 ± 1.1 to 4.8 ± 1.0µA, a mean 17% decrease, which corresponds to the usualslow run down of the ENaC current expressed in oocytes (Awaydaet al., 1996). Subsequent exposure to 2 µg/ml trypsininduced an increase of I_Na to 10.2 ± 2.1 µA, showingthat the oocytes were indeed able to react to trypsin as usual.

Effect on the Properties of ENaC
To test for the possibility of an alteration of the channelionic selectivity after trypsin treatment, we measured the amiloride-sensitivecurrent carried by Na⁺, Li⁺, or K⁺ before and after activationby trypsin. No significant amiloride-sensitive inward currentat –100 mV could be detected when K⁺ was the only extracellular monovalent cation before (0.02 ± 0.02 µA, n =6) or after a 5-min trypsin (2 µg/ml) treatment (0.03± 0.03 µA, n = 6). The amiloride-sensitive Na⁺channel has been shown to be more conductive for Li⁺ than for Na⁺ both in native tissue (Palmer and Frindt, 1988) and asthe result of ENaC expression in Xenopus oocyte (Canessa etal., 1994). We measured the amiloride-sensitive current in oocytesexpressing ${alpha}$ β ${gamma}$ XENaC before and after a 3-min exposure totrypsin. In 15 measurements, the mean Na current was 3.4 ±1.1 µA before and increased to 6.9 ± 1.4 µAafter trypsin treatment. The ratio of the amiloride-sensitivecurrent in 100 mM Na⁺ vs. 100 mM Li⁺ was 1.51 ± 0.05before trypsin, and decreased slightly to 1.44 ± 0.05after trypsin (P < 0.005, paired t test). We also measuredthe inhibitory constant (K_I) of amiloride before and aftera 3-min trypsin treatment in oocytes expressing ${alpha}$ β ${gamma}$ XENaCin the presence of 100 mM Na⁺, at –100 mV, according to the procedure used earlier (Puoti et al., 1995), using concentrations of 0.1, 1.0, 10, and 50 µM amiloride. In a group of 13 oocytes, I_Na increased about six times aftertrypsin treatment (from 1.09 ± 0.56 to 6.49 ±1.20 µA, P < 0.001), while the amiloride K_I did notchange significantly (0.55 ± 0.03 µM before vs.0.49 ± 0.03 µM after trypsin).

Role of Intracellular Calcium
As shown by Durieux et al. (1994), the first component of theresponse to trypsin, the chloride current, is dependent on arise of intracellular calcium. To evaluate the role of intracellularcalcium on the I_Na response to trypsin, we injected Xenopusoocytes expressing ${alpha}$ XENaC and β ${gamma}$ rENaC with 50 nl of 100 mMEGTA or water (control). As shown in the examples of Fig. 4and in accordance with Durieux et al. (1994), we found that this treatment abolished the transient chloride current, butit did not prevent the increase of the amiloride-sensitive current.In oocytes expressing ${alpha}$ β ${gamma}$ XENaC, trypsin induced a 5.6 ±1.2-fold increase (n = 9) in I_Na 10–20 min after EGTAinjection, a value similar to the mean 6.3 ± 1.2-foldincrease observed in control oocytes injected with water (n= 7) or noninjected oocytes (n = 4). In 10 oocytes expressingthe ${alpha}$ Xβr ${gamma}$ r ENaC and injected with EGTA, trypsin induced amean 14.5 ± 5.4-fold increase, which was not significantlydifferent from the effect observed without EGTA injection.

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Figure 4 Effect of intracellular EGTA injection. Original current recordings obtained in oocytes expressing ${alpha}$ XENaC and β ${gamma}$ rENaC. The current sensitive to 10 µM amiloride was measured at –100 mV before and after a 4-min exposure to 2 µg/ml trypsin. In these oocytes, the amiloride-sensitive sodium current (I_Na) is hardly detectable before trypsin treatment. (a) The recording obtained in a control oocyte injected with 50 nl of water before the electrophysiological measurement; a large transient current is observed almost immediately after trypsin treatment and a >20-fold increase in I_Na was induced. (b) The recording obtained with an oocyte injected with 50 nl of 200 mM EGTA; no transient Ca-activated Cl^– current could be observed, but the activation I_Na was similar to that observed in the absence of intracellular EGTA.

Relation with Regulation of ENaC through G Protein
To evaluate the potential role of G protein in the responseto trypsin, we followed the amiloride-sensitive current beforeand after trypsin treatment in oocytes injected with GTP- ${gamma}$ S,a nonspecific activator of all G proteins. As a positive control,we coexpressed human CFTR and the human β2 adrenergicreceptor and tested for activation of a chloride current by1 µM epinephrine. Epinephrine induced a fast increaseof the conductance in oocytes expressing CFTR and the β2 adrenergic receptor (Fig. 5 a). When oocytes were injectedwith GTP- ${gamma}$ S (0.09 nmol = 50 nl of a 1.8-mM GTP- ${gamma}$ S solution) 10–30min before the electrophysiological measurement, the initialconductance of the oocytes expressing CFTR was larger and theresponse to epinephrine was abolished (Fig. 5 b), indicatingthat GTP- ${gamma}$ S injection was efficient to activate G proteins.In contrast, when we studied oocytes expressing Xenopus ENaC,the baseline amiloride-sensitive current was similar in theGTP- ${gamma}$ S–injected and water-injected groups, and trypsininduced a large increase of the amiloride-sensitive current(Fig. 5 c) similar to that observed in the control group. Themean values of I_Na before and after trypsin and of the oocyteconductance (G) before and after epinephrine stimulation areshown in Fig. 5 d.

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Figure 5 Effect of G protein stimulation with GTP- ${gamma}$ S. (a) Original current recording showing the effect of 1 µM epinephrine on the conductance of an oocyte expressing the β-adrenergic receptor and CFTR. The holding potential was alternating between –40 and –60 mV with a 1 Hz frequency. (b) The same protocol was applied to an oocyte injected 13 min before with 50 nl of a 1.8-mM GTP- ${gamma}$ S solution. (c) Effect of trypsin (2 µg/ml for 3.5 min) on the amiloride-sensitive Na⁺ current (I_Na) at –100 mV after intracellular injection with GTP- ${gamma}$ S (50 nl, 1.8 mM). (d) The effect of a 3-min trypsin treatment (left) on I_Na(before trypsin, white bars; after trypsin, black bars) in oocytes expressing ${alpha}$ β ${gamma}$ XENaC. Nine oocytes were injected with GTP- ${gamma}$ S, and seven control oocytes were noninjected. The effect of trypsin was not affected by previous GTP- ${gamma}$ S intracellular injection. (right) The whole oocyte conductance in oocytes expressing CFTR and the β2-adrenergic receptor before (open bars) and after (filled bars) stimulation with 1 µM epinephrine. In control oocytes (n = 11) (i.e., without previous GTP- ${gamma}$ S injection), epinephrine induced an increase of the whole oocyte conductance (P < 0.005, paired t test). Intracellular GTP- ${gamma}$ S injection (n = 13) increased the oocyte conductance (P < 0.05, unpaired t test) and completely prevented the effect of epinephrine.

Effect of Trypsin and Channel Density
To evaluate the effect of trypsin on the number of channelsat the oocyte surface, we used channel mutants in which a FLAGepitope had been added to the extracellular domain of eachsubunit, and estimated the channel density by binding of iodinatedanti–FLAG antibody as described earlier (Firsov et al.,1996

). Anti– FLAG antibody binding was measured aftera 10-min exposure to trypsin (5 µg/ml) and in controloocytes not exposed to trypsin. At the same time, the amiloride-sensitivecurrent was measured in two parallel groups of oocytes exposedto the same treatment. The results of specific anti–FLAGbinding and the amiloride-sensitive current with or withouttrypsin treatment (shown in Fig. 6) indicate that trypsin doesnot induce a modification of the channel density at the cellsurface. Therefore, the increase in I_Na is not due to translocationof channels from an intracellular pool to the surface, and sothe increase in current must be due either to an increase insingle channel conductance or to a modification of the openprobability.

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Figure 6 Effect of trypsin on channel density. The channel density estimated by anti–FLAG antibody in oocytes injected with ${alpha}$ F, βF, and ${gamma}$ F ENaC cRNA (F indicates insertion of a FLAG epitope) was not modified by a 10-min exposure to trypsin (control group, n = 43; trypsin group, n = 44), indicating no effect of trypsin on the surface channel density, while the amiloride-sensitive Na current (I_Na) increased more than threefold in a parallel group of oocytes (P < 0.01, n = 24). For comparison, the effect of trypsin was tested in a group of oocytes injected with wild-type (without FLAG epitope) ${alpha}$ β ${gamma}$ rat ENaC in which there was no specific anti– FLAG antibody binding. Trypsin had a similar effect on I_Na in oocytes expressing the channel with FLAG epitope (middle columns) and in the wild-type channel (right columns).

Effect of Trypsin at the Single Channel Level
The effects of trypsin on the single channel current were examinedin Xenopus oocytes expressing ENaC using the cell-attached modeand excised patches in the outside-out configuration. Cell-attachedpatches were obtained using pipettes filled with a 100-mM LiClsolution with or without 5 µg/ml trypsin. Under theseconditions, typical Xenopus ENaC single channel currents (8pS inward current) were observed in 7 of 16 successful patches(44%) in the absence of trypsin and in 8 of 11 successful patches(73%) in the presence of trypsin. This difference is marginallysignificant (P < 0.05 by ${chi}$ ² test). Analysis of open probabilitydid not show obvious differences between the two groups, afact that is not surprising considering the very large spontaneousvariation in open probability observed with ENaC (Palmer andFrindt, 1988

, 1996

). To confirm the activation of the channelby trypsin, we took advantage of the observation, describedabove, that the heteromer composed of the ${alpha}$ subunit of Xenopusand the β and ${gamma}$ subunits of rat ENaC ( ${alpha}$ Xβr ${gamma}$ r) showeda much larger increase after trypsin treatment than either therat or Xenopus ${alpha}$ β ${gamma}$ ENaC. Channels were observed in 8 of 12successful patches (67%) when the pipette contained trypsin, but only in 1 of 16 successful patches (6%) without trypsin(P < 0.001). There was no difference in single channel conductancebetween any of these groups. The increase in active channeldensity observed in these experiments is consistent with thosefound in macroscopic current (see Table I).

Another series of experiments was carried out to test the possibilitythat trypsin could activate the sodium channel indirectly,for instance through the diffusion of a soluble intracellularsecond messenger. Patches in the cell-attached configurationwere obtained with LiCl solution–containing pipettes.The channel activity was recorded for 2–5 min under controlconditions, and then 5 µg/ml trypsin was added to thebath solution surrounding the pipette and the oocyte. A representativetrace is shown in Fig. 7 a. Although neither the absolute numberof channels nor the open probability could be determined accurately,there was no obvious increase in channel activity after perfusionwith trypsin. The mean values of the n.Po before and duringexposure to trypsin are given in Fig. 7 b. Together with the results obtained with trypsin in the pipette, these resultssuggest that the effect of trypsin is local (i.e., by actionof trypsin on the channel itself or on a closely associatedprotein) and is not mediated by a soluble intra-cellular secondmessenger.

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Figure 7 Effect of oocyte superfusion with trypsin on the Na⁺ channel activity. (a) Original channel recording showing the activity of Na⁺ channels in a cell-attached patch. At the time indicated by the bar, a solution containing 5 µg/ml trypsin was perfused around the oocyte. Trypsin did not induce any evident change in the channel activity. The pipette was filled with a solution containing 100 mM LiCl and the pipette potential was +100 mV. A downward deflection indicates current flowing from the pipette into the cell. The closed-channel level is indicated by the dotted line. (b) Mean Na⁺ channel activity expressed as n.Po in the absence and presence of the trypsin in the bath. Because of the large range and the highly asymmetrical distribution of the n.Po values, the mean n.Po was calculated as exp(mean(log(n.Po))). The control value is the mean n.Po over a 3-min period before trypsin and during each minute after superfusion with trypsin. The number of measurements is 16 for the control and 1-min values, and between 15 and 11 for the 2–5-min values.

We have also tested the effect of extracellular trypsin in the excised patch, outside-out configuration, with patches obtained on oocytes expressing Xenopus ${alpha}$ β ${gamma}$ ENaC. For theseexperiments, the pipette solution had the following composition(mM): 20 KCl, 80 K gluconate, 2 EGTA, 10 Na HEPES, pH 7.4,and the bath solution was a 100-mM LiCl solution, bufferedto pH 7.4 with 10 mM Na HEPES. Under these circumstances, wecould observe inward single channel currents, carried by lithium,at a holding potential V_pip of –100 mV. Most often afterpatch excision, there was either no channel activity or a rapidlyrunning down channel activity, but in a few cases a stablechannel activity was observed. In four such cases, the identityof the channel could be first verified by the effect of lowconcentration of external amiloride: 0.2 µM amilorideinduced a reversible decrease of n.Po to 45 ± 6% of itsinitial value (Fig. 8), a decrease compatible with the K_I 0.6µM observed for Xenopus ENaC in macroscopic current experiments(Puoti et al., 1995

). Trypsin (5 µg/ml) added to theextracellular side of the membrane did not induce any increase of the activity of ENaC (n.Po control 1.7 ± 1.0 vs.n.Po trypsin 1.2 ± 0.8, n = 4).

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Figure 8 Effect of extracellular trypsin on Na⁺ channel activity in outside-out excised patches. (a) In this original recording, amiloride (200 nM) added to the bath (extracellular side) solution, reduced the activity of a single Na⁺ channel, an effect that was quickly reversible. (b) With the same patch, trypsin (5 µg/ml) added to the external solution did not produce any obvious increase either in the single channel conductance or in the channel activity. The pipette was filled with a K⁺ gluconate solution and the bath solution contained 100 mM LiCl solution. The pipette potential was –100 mV. A downward deflection indicates a current flowing into the pipette and the closed-channel level is indicated by the dotted line. (c and d) The n.Po values in four patches in which recordings were obtained before, during, and after exposure to amiloride (c) and before and during exposure to trypsin (d) are shown.

	discussion

Top ABSTRACT introduction methods results discussion references

In contrast to several earlier reports indicating an inactivatingeffect of proteases on the epithelial sodium channel (Gartyand Edelman, 1983

; Lewis and Alles, 1986

; Lewis and Clausen,1991

), we have observed that trypsin and chymotrypsin inducea significant activation of the sodium or lithium current carriedby ENaC expressed in Xenopus oocytes. The stimulatory effectof proteases was obtained with much lower concentrations oftrypsin than those used in the experiments reported by Gartyand Edelman (1983)

or Lewis et al. (1991). Even using a largeconcentration of trypsin for a long time, we failed to observea decrease of the amiloride-sensitive Na⁺ current, suggestinga direct proteolytic degradation of the channel. The different experimental model, native tight epithelia versus Xenopus oocytesartificially expressing ENaC, might be the reason for thisdiscrepancy. In the oocyte, the expressed channel might be ina different conformation or be missing a protein componentdistinct from the ${alpha}$ , β, and ${gamma}$ subunits, a component thatmight be necessary for the sensitivity to the inhibitory effectof trypsin. Another difference is the species: we used ratand Xenopus ENaC, while the results published by Garty and Edelman (1983)

and Lewis et al. (1991) were obtained with Bufomarinus and rabbit tissues; minor sequence differences mightdetermine the presence or absence of a proteolytic site. Thishypothesis is supported by the observation of Jungwirth etal. (1991)

, who also failed to observe stimulatory effect oftrypsin or kallikrein on the transepithelial potential of ratdistal convoluted tubules.

The observation of a stimulatory effect of trypsin of the Na⁺current mediated by ENaC goes in the same direction as the observationof Orce et al. (1980) showing that inhibition by aprotininof a proteolytic activity in the apical medium from toad urinarybladder led to a reduced transepithelial sodium transport.The demonstration of the presence of a "kallikreinlike" protease activity in the apical medium of A6 cells grown on permeablesupport (Jovov et al., 1990) could well provide the physiologicalequivalent in a native epithelia of what we have observed withtrypsin and Na⁺ channels expressed in Xenopus oocytes. Thishypothesis has received strong support from the recent identificationof an endogenous serine protease naturally expressed in A6cells that is able to activate I_Na when coexpressed with ENaCin oocytes and the observation that trypsin also activatesthe electrogenic transepithelial Na⁺ transport in A6 cells providedthat the endogenous protease had first been inhibited (Valletet al., 1997). The experiments presented here give some firstindications about the mechanism by which a protease activefrom the extracellular side of the membrane might activate the Na⁺ channel.

The Effect of Trypsin Does Not Occur through G Protein-mediated Increase in cAMP or Intracellular Calcium
Trypsin is known to produce a transitory activation of calcium-activatedchloride current, an effect probably mediated by the activationof a G protein-coupled trypsin receptor naturally present atthe surface of the native oocyte, followed by activation ofphospholipase C, and IP3-mediates release calcium from endogenous calcium stores (Durieux et al., 1994). Several observationsindicate that the activation of the sodium current is not dueto the same mechanism. First, the chloride current can be preventedby intracellular calcium buffering, while the increase of theamiloride-sensitive current is not affected by this maneuver.Second, no detectable transient chloride currents were observedafter chymotrypsin treatment, suggesting that this enzyme was not able to activate the endogenous oocyte trypsin receptorwhile it produced a large increase in the Na⁺ current withboth Xenopus and rat ENaC. We therefore conclude that the ENaCresponse to proteases is not related to the presence of an oocyte-endogenoustrypsin receptor, but is mediated by a different mechanism than that responsible for the calcium-activated chloride currentresponse.

In amphibian and mammalian tight epithelia, the amiloride-sensitiveNa⁺ transport is stimulated by cAMP (Schafer and Hawk, 1992;Verrey, 1994) and this is the main mechanism by which vasopressincan increase the transepithelial Na⁺ transport. It was temptingto make the hypothesis that trypsin stimulation of I_Na in Xenopusoocytes occurred through the same mechanism, especially consideringthe similar time course of the responses (compare for instanceour data with the results obtained by Verrey, 1994, on A6 cells), but several observations indicate that this is not the case.First, I_Na, due to ENaC expression in Xenopus oocytes, doesnot appear to be stimulated by an increase of cAMP production(Awayda et al., 1996). Second, we could not modify the responseto trypsin by a pretreatment with GTP- ${gamma}$ S, which is a strong,although indirect, indication that no G proteins are involvedin the response of ENaC to trypsin.

Finally, the observation of the effect of trypsin on singleNa⁺ channel activity, in the "cell-attached" configuration,when trypsin was applied inside, but not outside, the pipette,indicated that the effect of trypsin is a "local" phenomenon;i.e., a mechanism that involves protein(s) that can be presenttogether with the channel within the $~$ 1 µm² of membranearea included in a patch and probably does not include thediffusion of a soluble second messenger.

All these data taken together indicate clearly that the effectof trypsin on the sodium current carried by ENaC is not mediatedby the "classical" pathway of receptor binding, G protein activation,second messenger production, protein kinase activation, orchannel phosphorylation.

Hypothetical Mechanism of Action of Trypsin on ENaC
The similar effects of two different serine proteases on theNa⁺ channel activity suggest that this effect is due to a proteolyticevent. The abolishment of the effect of trypsin by soybeantrypsin inhibitor is also compatible with this hypothesis.What might be the substrate of this proteolytic action?

The earlier published observations of an inhibitory effectof trypsin and other proteases on the epithelial Na⁺ channelhad demonstrated important modifications of the channel properties:change in selectivity (Lewis and Alles, 1986; Lewis and Clausen,1991) or inability to further respond to aldosterone (Gartyand Edelman, 1983). In addition, the effect of proteases couldbe prevented by the presence of an amiloride molecule in itsbinding site (Garty and Edelman, 1983; Schlichter et al., 1986).All these observations clearly supported the hypothesis thatthe channel itself (i.e., one of its protein components) wasthe substrate of the protease. Unfortunately, the situationis less clear concerning the stimulatory effect of trypsin.Although our results are all compatible with a direct effectof trypsin on one or several of the ENaC subunits, we couldnot find any direct evidence supporting this hypothesis. Theeffect of trypsin on the Na⁺/Li⁺ selectivity ratio is compatiblewith a modification of the selectivity filter of the channel,to which the "pre-M2" segment of each subunit seems to contribute(Schild et al., 1997). However, the observed change, althoughstatistically significant, is of such a small amplitude thatwe could not convince ourselves that this observation is areliable proof of the direct action of the protease on thechannel protein. The absence of modification of the Na⁺/ K⁺selectivity and of the affinity to amiloride does not supporta direct effect. Sodium channel activation by trypsin couldnot be blocked or even slowed down by a concentration of amiloridesufficient to occupy >95% of the channels. However, ourpatch clamp data clearly indicate a local effect. Therefore,the substrate of trypsin, if it is not the channel proteinitself, is probably a closely associated protein.

Although the effect of trypsin could be observed when appliedinside a patch pipette in the cell-attached mode, no effectof trypsin could be detected in excised outside-out patches.These observations should be interpreted with care because,due to the "run down" phenomenon, only a small fraction ofNa⁺ channels remain active in excised patches, and this fractionmay not be representative of the whole channel population; they nevertheless suggest that, although the proteolytic actionof trypsin is most probably extracellular, the activation processincludes some intracellular component that is disturbed bythe patch excision procedure. This situation is somewhat similarto that observed with the effect of vasopressin on the Na⁺channel density that could well be observed when the hormonewas applied before a patch was obtained, but not when vasopressin was added after the formation of a seal (Marunaka and Eaton,1991). However, in contrast with the well supported hypothesisof channel insertion for the response to vasopressin (Gartyand Palmer, 1997), our data obtained using FLAG insertion mutantsand anti– FLAG antibody binding do not support a significant change of surface channel density to explain the large increasein Na⁺ current density. Since the single channel conductancewas not modified, the effect of trypsin must be due to an increaseof the proportion of open channels in the total populationof channels present at the cell surface. Our data do not allowus to determine whether this increase results from a changein the open probability of already active channels or fromrecruitment out of a pool of completely silent channels. The large increase that is often observed after trypsin treatmentindicates that the overall open probability of all the channelspresent at the oocyte surface must be very low. As the meanopen probability of active channels observed in cell-attachedpatches on oocytes expressing ENaC is often of the order of0.5 (Canessa et al., 1994), our results suggest that theremay be a significant fraction of "silent" channels that arenot seen in patch clamp experiments, but are present at theoocyte surface and can be activated by proteolytic treatment.A similar conclusion was reached by Firsov et al. (1996) usingquantitative measurements of cell surface channel protein expression.The inverse relationship between the initial I_Na and the effectof trypsin (see Fig. 2) could be explained if there was a variabledegree of "spontaneous" activation, possibly by an oocyte-endogenousprotease. In oocytes with a low degree of spontaneous activation,trypsin would reveal a large portion of silent channels while,in oocytes with a high level of spontaneous activation, trypsincould only activate a small portion of silent channels.

In summary, trypsin or chymotrypsin can induce a large activationof the sodium channel obtained by expression of the ${alpha}$ , β,and ${gamma}$ subunits of the rat or Xenopus ENaC in Xenopus oocytes.This effect is due to an increase of the open probability ofchannels already present at the oocyte surface, through a proteolyticaction of the enzyme on the channel protein itself or a closelyassociated component.

¹ Abbreviations used in this paper: CFTR, cystic fibrosis transmembraneconductance regulator; ENaC, epithelial Na⁺ channel; I_Na, amiloride-sensitiveNa⁺ current.

ACKNOWLEDGMENTS

We are grateful to L. Schild, B. Rossier, and S. Cotecchia forcritical reading of the manuscript and for helpful suggestions.

This work was supported by the Human Frontier Science Program,grant RG-0464.

Submitted: 24 July 1997
Accepted: 15 October 1997

references

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ABSTRACT
introduction
methods
results
discussion
references

Awayda MS, Ismailov II, Berdiev BK, Fuller CM & Benos DJ. Protein kinase regulation of a cloned epithelial Na+ channel, J Gen Physiol, 1996, 108, 49–65.[Abstract/Free Full Text]

Canessa CM, Horisberger J-D & Rossier BC. Functional cloning of the epithelial sodium channel: relation with genes involved in neurodegeneration, Nature, 1993, 361, 467–470.[Medline]

Canessa CM, Schild L, Buell G, Thorens B, Gautshi Y, Horisberger J-D & Rossier BC. The amiloride-sensitive epithelial sodium channel is made of three homologous subunits, Nature, 1994, 367, 463–467.[Medline]

Durieux ME, Salafranca MN & Lynch KR. Trypsin induces Ca²⁺-activated Cl^– currents in X. laevisoocytes, FEBS Lett, 1994, 337, 235–238.[Medline]

Firsov D, Schild L, Gautschi I, Merillat AM, Schneeberger E & Rossier BC. Cell surface expression of the epithelial Na channel and a mutant causing Liddle syndrome—a quantitative approach, Proc Natl Acad Sci USA, 1996, 93, 15370–15375.[Abstract/Free Full Text]

Garty H & Edelman IS. Amiloride-sensitive trypsinization of apical sodium channels. Analysis of hormonal regulation of sodium transport in toad bladder, J Gen Physiol, 1983, 81, 785–803.[Abstract/Free Full Text]

Garty H & Palmer LG. Epithelial sodium channels— function, structure, and regulation, Physiol Rev, 1997, 77, 359–396.[Abstract/Free Full Text]

Hamill OP, Marty A, Neher E, Sakmann B & Sigworth FJ. Improved patch-clamp technique for high-resolution current recording from cells and cell-free membrane patches, Pflügers Arch, 1981, 391, 85–100.[Medline]

Jovov B, Wills NK, Donaldson PJ & Lewis SA. Vectorial secretion of a kallikrein-like enzyme by cultured renal cells. I. General properties, Am J Physiol, 1990, 259, C869–C882.[Medline]

Jungwirth A, Lewis S & Lang F. Kallikrein does not modify the transepithelial potential of rat renal distal convoluted tubules, Nephron, 1991, 58, 225–228.[Medline]

Lewis SA & Alles WP. Urinary kallikrein: a physiological regulator of epithelial Na absorption, Proc Natl Acad Sci USA, 1986, 83, 5345–5348.[Abstract/Free Full Text]

Lewis SA & Clausen C. Urinary proteases degrade epithelial sodium channels, J Membr Biol, 1991, 122, 77–88.[Medline]

Marunaka Y & Eaton DC. Effects of vasopressin and cAMP on single amiloride-blockable Na channels, Am J Physiol, 1991, 260, C1071–C1084.[Medline]

Methfessel C, Witzemann V, Takahashi T, Mishina M, Numa S & Sakmann B. Patch clamp measurements on Xenopus laevis oocytes: currents through endogenous channels and implanted acetylcholine receptor and sodium channels, Pflügers Arch, 1986, 407, 577–588.[Medline]

Orce GG, Castillo GA & Margolius HS. Inhibition of short-circuit current in toad urinary bladder by inhibitors of glandular kallikrein, Am J Physiol, 1980, 239, F459–F465.[Medline]

Palmer LG & Frindt G. Conductance and gating of epithelial Na channels from rat cortical collecting tubule, J Gen Physiol, 1988, 92, 121–138.[Abstract/Free Full Text]

Palmer LG & Frindt G. Gating of Na channels in the rat cortical collecting tubule: effects of voltage and membrane stretch, J Gen Physiol, 1996, 107, 35–45.[Abstract/Free Full Text]

Puoti A, May A, Canessa CM, Horisberger J-D, Schild L & Rossier BC. The highly selective low conductance epithelial Na channel of Xenopus laevisA6 kidney cells, Am J Physiol, 1995, 38, C188–C197.

Schafer JA & Hawk CT. Regulation of Na⁺channels in the cortical collecting duct by AVP and mineralocorticoids, Kidney Int, 1992, 41, 255–268.[Medline]

Schild L, Schneeberger E, Gautschi I & Firsov D. Identification of amino acid residues in the ${alpha}$ , β, and ${gamma}$ subunits of the epithelial sodium channel (ENaC) involved in amiloride block and ion permeation, J Gen Physiol, 1997, 109, 15–26.[Abstract/Free Full Text]

Schlichter L, Sidell N & Hagiwara S. K channels are expressed early in human T-cell development, Proc Natl Acad Sci USA, 1986, 83, 5623–5629.

Vallet V, Chraibi A, Gaeggeler H-P, Horisberger J-D & Rossier BC. An epithelial serine protease activates the amiloride-sensitive sodium channel, Nature, 1997, 389, 607–610.[Medline]

Verrey F. Antidiuretic hormone action in A6 cells: effect on apical Cl and Na conductances and synergism with aldosterone for NaCl reabsorption, J Membr Biol, 1994, 138, 65–76.[Medline]

Zhou H, Tate SS & Palmer LG. Primary structure and functional properties of an epithelial K channel, Am J Physiol, 1994, 35, C809–C824.[Medline]

Zweifach A & Lewis SA. Characterization of a partially degraded Na+ channel from urinary tract epithelium, J Membr Biol, 1988, 101, 49–56.[Medline]

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