Uptake and Release of [3H]Formycin B via Sodium-Dependent Nucleoside Transporters in Mouse Leukemic L1210/MA27.1 Cells

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Vol. 281, Issue 1, 347-353, 1997

Uptake and Release of [³H]Formycin B via Sodium-Dependent Nucleoside Transporters in Mouse Leukemic L1210/MA27.1 Cells¹

Stephanie L. Borgl and and Fiona E. Parkinson

Department of Pharmacology and Therapeutics, University of Manitoba, Winnipeg, Manitoba, Canada

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

At least seven functionally distinct nucleoside transport processes exist; however, mouse leukemic L1210/MA27.1 cells possessonly one subtype, a Na⁺-dependent transporter termed N1/cif. The capacity of this transportersubtype to release nucleosides from L1210/MA27.1 cells was investigatedwith the poorly metabolized inosine analog [³H]formycin B. Uptake of [³H]formycin B into these cells was inhibited by replacement ofNa⁺ in the buffer with choline, or by blocking Na⁺/K⁺ ATPase with 2 mM ouabain, inhibiting glycolysis with 5 mM iodoaceticacid or inhibiting nucleoside transport with 1 mM phloridzin.Sodium stimulated uptake with an EC₅₀ value of 12 mM. To measurerelease of [³H]formycin B, cells were loaded with [³H]formycin B (10 µM) then washed and resuspended in buffer. Replacementof Na⁺ in the buffer with choline enhanced [³H]formycin B release by 20 to 47%, and significant stimulationof release was observed with Na⁺ concentrations of 30 mM or less. Resuspending loaded cells intoNa⁺ buffer containing 2 mM ouabain or 10 µM monensin, a Na⁺ ionophore, significantly enhanced [³H]formycin B release during 20 min by 39% or 29%, respectively.Release of [³H]formycin B into choline buffer was inhibited 26.5% by 10 mMphloridzin and 39.6% by 10 mM propentofylline, compounds knownto inhibit various transporters including Na⁺-dependent nucleoside transporters. Release was also inhibitedsignificantly by 100 µM concentrations of dilazep, dipyridamoleand nitrobenzylthioinosine, inhibitors with selectivity for Na⁺-independent nucleoside transporters. In the absence of Na⁺, the permeants adenosine and uridine enhanced [³H]formycin B release by up to 40.9% and 21.4%, respectively. Thesedata indicate that in the absence of an inwardly directed Na⁺ gradient, Na⁺-dependent nucleoside transporters can function in the releaseof nucleosides.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Nucleoside transport processes are membrane-bound carrier proteins that mediate the transfer of nucleosides across plasmamembranes. Seven transporters have been characterized accordingto function (Cass, 1995) and are divided into two broad classes:Na⁺-independent and Na⁺-dependent processes. Na⁺-independent transporters are facilitated diffusion processesthat catalyze cellular influx or efflux of nucleosides with thedirection of movement determined by the nucleoside concentrationgradient. Two equilibrative transporters are distinguished bytheir sensitivity to the transport inhibitor NBMPR and are termedequilibrative sensitive (es) and equilibrative insensitive (ei),respectively (Vijayalakshmi and Belt, 1988). Na⁺-dependent transporters couple the influx of Na⁺ to the influx of nucleosides; thus, in the presence of a transmembraneNa⁺-gradient nucleosides can be concentrated within cells to levelsin excess of those in the extracellular environment. Five Na⁺-dependent nucleoside transporters have been described and aretermed N1 to N5. N1, also called cif, accepts purines and uridineas permeants, whereas N2, also called cit, and N4 are pyrimidineselective. N3 and N5, also called cib and cs, respectively, havebroad permeant selectivity and accept both purines and pyrimidines.N5 (cs) is unique among the currently identified Na⁺-dependent transporters for its sensitivity to inhibition by lownanomolar concentrations of NBMPR. Dipyridamole and dilazep inhibitboth es and ei but are poor inhibitors of Na⁺-dependent transporters (Cass, 1995).

Nucleoside transport processes are an important component of nucleoside salvage pathways and provide cells with nucleosidesthat are required for cellular metabolism. In addition, adenosineis an endogenous nucleoside that has autocrine and paracrine regulatoryeffects. In brain, adenosine is an inhibitory neuromodulator,and extracellular adenosine levels are regulated by nucleosidetransport processes. Recent evidence indicates that glutamatetransporters, which are dependent on Na⁺ and normally function in cellular uptake, can mediate glutamaterelease after depolarization, ATP depletion or glycolytic inhibition(Madl and Burgesser, 1993; Gemba et al., 1994). It has been proposedthat this is an important source of extracellular glutamate duringconditions of abnormal metabolism, such as stroke (Szatkowskiand Attwell, 1994). Because adenosine levels also increase duringstroke and cellular release of adenosine can be resistant to inhibitorsof es and ei transporters (Geiger and Fyda, 1991), we investigatedwhether Na⁺-dependent nucleoside transporters can mediate nucleoside releaseduring conditions that perturb transmembrane Na⁺ gradients.

Murine leukemia L1210 cells possess both Na⁺-independent (es and ei) and Na⁺-dependent (N1/cif) nucleoside transporter activities (Crawfordet al., 1990b). Mutation strategies led to the isolation of L1210/MA27.1cells which retain only an N1/cif nucleoside transporter (Crawfordet al., 1990a); thus, these cells provide a model system to examinethe function of Na⁺-dependent nucleoside transporters. We investigated cellular releaseof [³H]formycin B, a poorly metabolized inosine analog (Plagemann etal., 1990; Dagnino and Paterson, 1990; Wu et al., 1993) that isa permeant of N1/cif transporters present in L1210/MA27.1 cells(Crawford et al., 1990a), and found evidence for Na⁺-dependent transporter-mediated release of [³H]formycin B.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Materials. Mouse leukemic L1210/MA27.1 cells were provided by Dr. J.A. Belt. [³H]Formycin B was purchased from Moravek Biochemicals (Brea, CA).[³H]Adenosine, ³H₂O and [³H]polyethylene glycol were from DuPont NEN (Boston, MA). NBMPRwas obtained from Research Biochemicals International (Natick,MA). RPMI 1640 and heat-inactivated horse serum were purchasedfrom Gibco BRL (Burlington, Ontario). Dilazep was provided byF. Hoffmann-LaRoche Ltd (Basel, Switzerland). All other reagentswere obtained from Sigma Chemical Co. (St. Louis, MO).

Cell culture. Mouse leukemic L1210/MA27.1 cells were maintained in logarithmic phase growth in RPMI 1640 culture medium with 10% heat-inactivatedhorse serum. Cells were harvested by centrifugation at 100 × gfor 10 min, washed twice with Na⁺ buffer (in mM: NaCl, 118; KCl, 4.9; MgCl₂, 1.2; KH₂PO₄, 1.4;4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid, 25; glucose,11; CaCl₂, 1; pH 7.4, 300 ± 10 mOsm) then resuspended in Na⁺ buffer to 10⁶ cells/ml. For some experiments, cells were washed and resuspendedin buffer in which NaCl was replaced with equimolar choline chloride(choline buffer). For experiments with iodoacetic acid, glucosewas omitted from the buffer. Osmolarity of buffers was adjusted,as necessary, to 300 ± 10 mOsm with NaCl or choline chloride.

Measurements of [³H]formycin B uptake. [³H]Formycin B (10 µM; 6 µCi/ml) uptake into L1210/MA27.1 cells was measured by an oil-stop centrifugation method as describedpreviously (Parkinson et al., 1993).

The effect of ouabain, an inhibitor of Na⁺/K⁺ ATPase, iodoacetic acid, an inhibitor of glycolysis, or phloridzin, an inhibitorof Na⁺-dependent nucleoside transport (Lee et al., 1990

), on [³H]formycin B uptake was assessed. Cells were preincubated with2 mM ouabain for 40 min at 37°C (Dagnino et al., 1991

), 5 mM iodoaceticacid for 20 min at 37°C (Plagemann and Aran, 1990

) or 1 mM phloridzinfor 15 min at 22°C (Huang et al., 1993

) and [³H]formycin B uptake (22°C) was determined. The effect of nucleosidetransport inhibitors on [³H]formycin B uptake was determined with cells preincubated for15 min (22°C) with 100 µM concentrations of NBMPR, dilazep ordipyridamole.

The effect of graded Na⁺ concentrations on [³H]formycin B uptake was determined by preparing and incubating (15 min, 22°C) cellsin buffers containing 0, 6, 12, 30, 59 or 118 mM NaCl. Aliquotsof cells were added to reaction mixtures containing [³H]formycin B in identical Na⁺ concentrations. After uptake intervals of 180 sec, reactionswere terminated and cell-associated radioactivity was determined.

Measurements of [³H]formycin B release. Cells were washed and resuspended at 5 × 10⁶ cells/ml in Na⁺ buffer and loaded with 10 µM (1 µCi/ml) [³H]formycin B for 30 or 70 min at 37°C. To determine total cellularloading of [³H]formycin B, aliquots of cells (100 µl) were centrifuged (13,000× g) through oil and associated radioactivity was determined.To assay cellular release of [³H]formycin B, 100-µl aliquots of cells were transferred to 1.5-mlmicrocentrifuge tubes, centrifuged (13,000 × g) for 5 sec andloading buffer was aspirated. Cell pellets were cooled on iceand then resuspended in either Na⁺ or choline buffer (22°C; 500 µl), and 400-µl aliquots were transferredto 1.5-ml microcentrifuge tubes containing 200 µl oil. After releaseintervals of 1 to 20 min, cells were centrifuged through oil andboth supernatants (350 µl) and cell pellets were analyzed forradioactivity. Cells resuspended into buffer at 4°C were usedto estimate release at 0 min. Cell viability after resuspensionwas determined by trypan blue exclusion assays and was routinelygreater than 95%.

The effect of extracellular Na⁺ concentrations on [³H]formycin B release was determined by resuspending [³H]formycin B-loaded cells in 4°C or 37°C buffer containing 0,30, 59 or 118 mM NaCl. Values of release at 0 min were subtractedfrom 10- and 20-min release values for each buffer.

To determine the effects of ouabain, iodoacetic acid or the Na⁺-ionophore monensin on [³H]formycin B release, cells loaded for 30 min with [³H]formycin B were resuspended in Na⁺ buffer (4°C or 37°C) alone or in Na⁺ buffer containing 2 mM ouabain, 10 µM monensin or 5 mM iodoaceticacid. Release of [³H]formycin B during time intervals of 0, 10 or 20 min was measuredas described above. To test whether these treatments affectedcell viability, trypan blue dye exclusion or intracellular watervolume was measured. To determine intracellular volume, cellswere incubated in Na⁺ buffer for 30 min at 37°C, centrifuged and resuspended in bufferas described above. After 20 min at 37°C, ³H₂O (0.7 µCi/ml) or [³H]polyethylene glycol (0.7 µCi/ml) was added and cells were incubatedfor a further 3 min. Cells were then centrifuged through oil andcell pellets were assayed for tritium content.

The effects of inhibitors or permeants of nucleoside transport processes on release of [³H]formycin B were evaluated. Cells were loaded with [³H]formycin B in Na⁺ buffer for 30 min at 37°C. Cell aliquots (100 µl) were centrifuged(13,000 × g) for 5 sec, supernatants were removed and pelletswere resuspended in 500 µl choline buffer in the absence or presenceof the nucleoside transport inhibitor phloridzin, dilazep, dipyridamole,NBMPR or propentofylline, or in the absence or presence of theN1/cif transporter permeant adenosine or uridine. Cells were incubatedfor 10 or 20 min at 37°C and then centrifuged through oil.

Measurements of [³H]adenosine release. The effect of iodoacetic acid on [³H]adenosine release was determined as described above, with cells loaded for 30 min (37°C)with [³H]adenosine (10 µM; 1 µCi/ml).

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Cellular accumulation of [³H]formycin B in L1210/MA27.1 cells. Cellular uptake of [³H]formycin B was greater with cells in Na⁺ buffer than with cells in choline buffer; the rates of uptakewere 7.6 ± 0.3 pmol/10⁶ cells/min and 0.2 ± 0.4 pmol/10⁶ cells/min, respectively. For cells in Na⁺ buffer, uptake of [³H]formycin B was reduced by treatment of the cells with 2 mM ouabain,5 mM iodoacetic acid or 1 mM phloridzin; the rates of uptake were1.5 ± 0.2, 1.8 ± 0.4 and 0.6 ± 0.3 pmol/10⁶ cells/min, respectively (fig. 1). Uptake of [³H]formycin B was inhibited 23.6% by 100 µM NBMPR, 59.2% by 100µM dilazep and 56.6% by 100 µM dipyridamole (data not shown).Sensitivity of [³H]formycin B uptake to Na⁺ was determined by measuring cellular accumulation in the presenceof graded concentrations of NaCl. The EC₅₀ value obtained by nonlinearregression analysis was 12 mM Na⁺ (fig. 2).

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Fig. 1. Cellular accumulation of [³H]formycin B in L1210/MA27.1 cells. Cells were harvested, then washed and resuspended in Na⁺ (closed symbols) or choline (open squares) buffer. Cells wereincubated with [³H]formycin B (10 µM) in buffer alone (squares) or in Na⁺ buffer containing 2 mM ouabain (closed triangles), 5 mM iodoaceticacid (closed circles) or 1 mM phloridzin (closed diamonds). Symbolsrepresent means and bars represent S.E. for three separate experiments,each performed in quadruplicate.

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Fig. 2. Effect of extracellular Na⁺ concentration on [³H]formycin B uptake by L1210/MA27.1 cells. Cells were harvested, washed and thenresuspended in buffer containing 0, 6, 12, 30, 59 or 118 mM NaCl.Choline chloride was added to maintain constant osmolarity. Uptakeof [³H]formycin B during 180-sec intervals was measured. Symbols representmeans and bars represent S.E. of three experiments performed inquadruplicate.

Release of [³H]formycin B from L1210/MA27.1 cells. Total [³H]formycin B loaded in 70 min was 99,000 ± 12,000 dpm/10⁶ cells (mean ± S.D.; n = 2). Release was stimulated by resuspendingcells in Na⁺ or choline buffer at 22°C. During 10-min intervals, the percentof total loaded [³H]formycin B that was released into Na⁺ or choline buffer was 31 ± 4% (mean ± S.D.) or 53 ± 7%, respectively(fig. 3). The rate of release of [³H]formycin B at 22°C was 3.2 ± 0.3 pmol/5 × 10⁶ cells/min in choline buffer and 1.1 ± 0.2 pmol/5 × 10⁶ cells/min in Na⁺ buffer (fig. 3).

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Fig. 3. Effect of extracellular Na⁺ on release of [³H]formycin B from L1210/MA27.1 cells. Cells were loaded with [³H]formycin B in Na⁺ buffer for 70 min (37°C). Cells were centrifuged briefly (5 sec,13,000 × g) and extracellular [³H]formycin B was removed. Cells were resuspended in Na⁺ (filled circles) or choline (filled squares) buffer at 22°C.Release was terminated by centrifuging cells through oil. Symbolsrepresent means and bars represent S.D. of two separate experiments,performed in quadruplicate.

Total [³H]formycin B loaded in 30 min was 90,000 ± 3,000 dpm/10⁶ cells (mean ± S.E.; n = 26). Release of [³H]formycin B was examined at 37°C in the presence of several concentrationsof Na⁺. No effect of Na⁺ concentration on release at 0 min was apparent (data not shown);however, release at 10 or 20 min in buffer containing 118 mM Na⁺ was significantly (P < .05, ANOVA with Tukey's HSD post tests)less than release in buffers containing 0 or 30 mM Na⁺ (fig. 4). The percent of total loaded [³H]formycin B that was released into Na⁺ buffer (118 mM NaCl) during 0, 10 or 20 min was 16 ± 1%, 54 ±1%, and 65 ± 1%, respectively. Release during 10 or 20 min (37°C)was 47% or 20% greater in buffer containing 118 mM choline chloridethan in buffer containing 118 mM NaCl (fig. 4).

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Fig. 4. Effect of Na⁺ concentration on release of [³H]formycin B from L1210/MA27.1 cells. Cells were incubated with [³H]formycin B for 30 min (37°C) in the presence of Na⁺. Cells were pelleted (5 sec; 13,000 × g) and extracellular [³H]formycin B was removed. Cells were resuspended in buffers containing0, 30, 59 or 118 mM NaCl at 37°C and incubated for 10 (open bars)or 20 min (closed bars) before pelleting through oil (30 sec;13,000 × g). Release of [³H]formycin B at 0 min was estimated with cells resuspended intobuffers at 4°C and was 31.6 to 34.7 pmol. Values for 0 min weresubtracted from values for 10- and 20-min release intervals. Barsrepresent S.E. of three separate experiments performed in quadruplicate.(*P < .05 ANOVA with Tukey's HSD post test comparing [³H]formycin B released in the presence of 0, 30 or 59 mM NaCl to[³H]formycin B released at 118 mM NaCl).

Release of [³H]formycin B was enhanced by treatment of loaded cells with 2 mM ouabain or 10 µM monensin for 10 or 20 min (fig.5). After 20 min treatment with ouabain or monensin, release of[³H]formycin B was significantly (P < .05, paired t test) increasedby 39% or 29%, respectively. In contrast, release was inhibitedby treatment with 5 mM iodoacetic acid (fig. 5). Release was significantly(P < .05, paired t test) inhibited by 35% relative to control,after 20 min exposure to 5 mM iodoacetic acid (fig. 5). Becausethe glycolytic inhibitor iodoacetic acid may elevate endogenousadenosine levels, which could then competitively inhibit releaseof [³H]formycin B, we tested the effect of iodoacetic acid treatmenton tritium release after loading of cells with [³H]adenosine (fig. 6). After 10- or 20-min treatments with iodoaceticacid, tritium release was significantly increased by 303% or 364%,respectively. Ouabain, monensin or iodoacetic acid treatment hadno significant effect on intracellular volume or on cell viability(data not shown).

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Fig. 5. Effect of ouabain, monensin or iodoacetic acid on release of [³H]formycin B from L1210/MA27.1 cells. Cells were loaded with [³H]formycin B (10 µM) in Na⁺ buffer for 30 min (37°C). Cells were centrifuged briefly (5 seconds,13,000 × g) and extracellular [³H]formycin B was removed. Cells were resuspended into Na⁺ buffer (37°C) in the absence (open bars) or presence (filledbars) of 2 mM ouabain (top panel), 10 µM monensin (center panel)or 5 mM iodoacetic acid (lower panel). Tritium content of supernatantswas measured 10 or 20 min after resuspension. [³H]Formycin B content of supernatants at 0 min, determined by resuspendingcells into Na⁺ buffer (4°C) in the absence or presence of ouabain, monensinor iodoacetic acid, was subtracted from 10- and 20-min values.Bars represent S.E. for three separate experiments performed inquadruplicate (*P < .05, paired t test comparing [³H]formycin B release in the presence and absence of inhibitor).

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Fig. 6. Effect of iodoacetic acid on release of [³H]adenosine from L1210/MA27.1 cells. Cells were loaded with 10 µM [³H]adenosine in Na⁺ buffer for 30 min (37°C). Cells were centrifuged briefly (5 sec,13,000 × g) and extracellular tritium was removed. Cells wereresuspended into Na⁺ buffer (37°C) in the absence (open bars) or presence (filledbars) of 5 mM iodoacetic acid. Tritium content of supernatantswas measured 10 or 20 min after resuspension. Tritium contentof supernatants at 0 min was determined by resuspending cellsinto Na⁺ buffer (4°C) in the absence or presence of iodoacetic acid andwas subtracted from values for 10- and 20-min release intervals.Bars represent S.E. for three separate experiments performed inquadruplicate. (*P < .05, **P < .01; paired t test comparing tritiumrelease in the presence and absence of iodoacetic acid).

Inhibitors of nucleoside transport processes were examined for effects on [³H]formycin B release from L1210/MA27.1 cells (table 1), and significantinhibition of [³H]formycin B release was observed with each of the transport inhibitorsused. Phloridzin, which inhibits nucleoside uptake by Na⁺-dependent but not by Na⁺-independent nucleoside transporters, produced significant inhibitionof [³H]formycin B release only at 10 mM, the highest concentrationused. Propentofylline, which can inhibit adenosine uptake by bothNa⁺-dependent and Na⁺-independent nucleoside transporters, significantly inhibited[³H]formycin B release at both 1 and 10 mM. The classical inhibitorsof Na⁺-independent nucleoside transport, dipyridamole, NBMPR and dilazep,also produced significant inhibition of [³H]formycin B release; at 100 µM concentrations release was inhibitedby approximately 10% with dilazep and 25% with NBMPR or dipyridamole.At concentrations of 10 µM, dipyridamole and NBMPR inhibited releaseby 0 to 10%. Of the inhibitors tested and at the concentrationsused, propentofylline produced the greatest inhibition of release(38%).

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TABLE 1
Effect of nucleoside transport inhibitors on release of [³H]formycin B.
Cells were loaded with [³H]formycin B, extracellular tritium was removed and cells were resuspended in choline buffer (37°C)in the absence or presence of test compounds. After 10- or 20-minrelease intervals, the tritium content of supernatants was determined.[³H]Formycin B released in the presence of inhibitors is expressedas a percent of control release, determined in the absence ofadded compounds. Experiments consisted of controls and two drugconcentrations, and they were performed in quadruplicate and repeatedat least three times.

The effect of the nucleoside transporter permeants, adenosine and uridine, on release of [³H]formycin B was tested (table 2). In contrast to the inhibitoryeffects of nucleoside transport inhibitors, release of [³H]formycin B during 10 or 20 min exposure to adenosine or uridineat concentrations of 100 µM to 10 mM was significantly greaterthan release in choline buffer alone. At 10 µM, the lowest concentrationtested, release was significantly greater than control after 20min, but not 10 min, exposure to adenosine or uridine. At concentrationsof 100 µM to 10 mM, adenosine produced greater elevation of [³H]formycin B release than did uridine.

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TABLE 2
Effect of the nucleosides adenosine and uridine on release of [³H]formycin B
Cells were loaded with [³H]formycin B, extracellular tritium was removed and cells were resuspended in choline buffer in theabsence or presence of test compounds. After 10- or 20-min releaseintervals, tritium content of supernatants was determined. [³H]Formycin B released in the presence of nucleoside is expressedas a percent of control release which was determined in the absenceof nucleoside. Experiments, consisting of controls and two drugconcentrations, were performed in quadruplicate and repeated atleast three times.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The main finding of this study was that release of [³H]formycin B from L1210/MA27.1 cells was Na⁺ dependent; removal of extracellular Na⁺ or disruption of transmembrane Na⁺ gradients enhanced [³H]formycin B release.

As shown previously (Parkinson et al., 1993; Crawford et al., 1990a), uptake of nucleosides by mouse leukemic L1210/MA27.1cells, was inhibited by removal of extracellular Na⁺. In the presence of physiological levels of Na⁺, the uptake of [³H]formycin B during a 5-min interval was 5-fold greater than inthe absence of Na⁺. An EC₅₀ value of 12 mM Na⁺ was obtained, which agrees with the value (13 mM) for nucleosidetransporter-mediated uptake of 6-mercaptopurine in rat intestinalbrush-border membrane vesicles (Iseki et al., 1996). Phloridzin,an inhibitor of Na⁺-dependent transporters for glucose as well as those for nucleosides(Lee et al., 1988, 1990), inhibited [³H]formycin B uptake by 73% over 5 min. Disruption of transmembraneNa⁺ gradients by blocking Na⁺/K⁺ ATPase activity with ouabain or by depressing cellular ATP storeswith the glycolytic inhibitor iodoacetic acid decreased [³H]formycin B uptake to 30 to 35% of control.

After loading of cells with [³H]formycin B, release was enhanced by removal of extracellular Na⁺, or by treating cells with phloridzin, ouabain or monensin, whichindicated that nucleoside release from these cells is stimulatedby conditions that perturb transmembrane Na⁺ gradients.

In contrast to the stimulatory effects of ouabain, monensin and Na⁺ replacement, the glycolytic inhibitor iodoacetic acid decreased[³H]formycin B release. By depressing intracellular ATP levels,iodoacetic acid can depress Na⁺/K⁺ ATPase activity and cause intracellular Na⁺ overload (Gemba et al., 1994); and it would thus be expectedto have effects on nucleoside release similar to those of ouabainand monensin. We hypothesized that, by depressing ATP levels,iodoacetic acid elevated levels of intracellular adenosine whichthen competitively inhibited release of [³H]formycin B. Consistent with this hypothesis, we found that iodoaceticacid stimulated tritium release in cells loaded with [³H]adenosine. The difference in release of these two compoundsindicates that [³H]adenosine is the better permeant for outward transport. Previously,it had been shown that Na⁺-dependent influx of 1 µM adenosine (190 pmol/10⁹ cells/sec) was approximately 8-fold faster than that of 1 µMformycin B (24 pmol/10⁹ cells/sec) in L1210 cells (Crawford et al., 1990b) and that adenosinehas greater affinity than formycin B for N1/cif transporters (Vijayalakshmiand Belt 1988).

An interesting finding of these studies was that treatment of cells with phloridzin, ouabain or Na⁺-replacement buffer was more effective in inhibiting [³H]formycin B uptake than in stimulating [³H]formycin B release. At least three factors may contribute tothis difference. First, each of these treatments may elevate intracellularadenosine levels. In this case, total nucleoside release may beunderestimated by measuring [³H]formycin B release, because simultaneous release of nonradioactiveadenosine may competitively inhibit [³H]formycin B release. Second, uptake studies were performed withcells pretreated with the desired buffers and drugs; however,because pretreatment was not possible for release studies, releasewas measured from the beginning of exposure of cells to the varioustreatment conditions. Because the drugs were not at equilibrationwith their respective target sites before initiation of release,this could lead to underestimation of the effects of the celltreatments on [³H]formycin B release. Third, the finite intracellular volume ofthe cells meant that intracellular [³H]formycin B concentrations were not constant for the durationof the release intervals. Each of these three factors would havethe effect of lowering [³H]formycin B release.

Differences were also observed in the Na⁺ concentration dependence of [³H]formycin B uptake and release; for example, uptake was unaffectedbut release was stimulated by reducing the buffer Na⁺ concentration from physiological to 30 mM. This may indicatethat intracellular levels of Na⁺ are higher in cells used for release assays than in cells usedfor uptake assays. It is possible that intracellular Na⁺ levels are elevated before initiation of release intervals, becausecells are loaded with [³H]formycin B in the presence of Na⁺ buffer.

Release of [³H]formycin B was depressed by millimolar concentrations of low-affinity inhibitors of Na⁺-dependent nucleoside transporters, such as propentofylline (Parkinsonet al., 1993) and phloridzin (Lee et al., 1988, 1990). Releasewas also decreased by 10 to 100 µM concentrations of NBMPR, dipyridamoleand dilazep, inhibitors that at nanomolar concentrations are selectivefor Na⁺-independent nucleoside transporters (Cass, 1995). Several studieshave measured adenosine release in the presence or absence ofNBMPR or dipyridamole at concentrations of 10 to 100 µM (Hoehnand White, 1990; Craig and White, 1993; Green, 1980; Cunha etal., 1996). Inhibition of release has been interpreted as evidenceof release mediated by equilibrative transporters. However, thepresent study indicates that NBMPR, dipyridamole and dilazep caninhibit nucleoside uptake and release mediated by Na⁺-dependent transporters. Thus, high (>10 µM) concentrations ofthese compounds should be used with caution in investigationsof cellular release mechanisms for nucleosides.

Stimulation of release by adenosine and uridine may indicate transacceleration in the absence of a Na⁺ gradient. This phenomenon, commonly observed with Na⁺-independent nucleoside transporters (Jarvis, 1986), can occurwhen transporter permeants are simultaneously present on bothsides of the membrane. In the presence of a Na⁺-gradient, Na⁺-dependent transporters function as symporters and translocatenucleosides in an inward direction. As long as the Na⁺ gradient is maintained, the intracellular accumulation of permeantsdoes not appear to affect permeant uptake. Our data suggest, however,that disruption of transmembrane Na⁺ gradients may uncouple nucleoside transport from Na⁺ translocation, and in this situation transport of nucleosidesin one direction may accelerate the transfer in the opposite direction.

Carrier-mediated release of neurotransmitters, including glutamate, $gamma$ -aminobutyric acid and dopamine, has been demonstratedby elevating intracellular Na⁺ levels, replacing extracellular Na⁺, blocking Na⁺/K⁺ ATPase activity or inhibiting glycolysis (Gemba et al., 1994;Eshleman et al., 1994; Levi and Raiteri, 1993; Belhage et al.,1993). Furthermore, it has been suggested that carrier-mediatedrelease of glutamate is a significant source of excitotoxic extracellularglutamate in cerebral ischemia (Szatkowski and Attwell, 1994).Adenosine released via reversal of Na⁺-dependent nucleoside transporters may contribute to the micromolarlevels of extracellular adenosine that arise during cerebral ischemia.Molecular evidence indicates that mRNA for N1/cif and N2/cit transportersis widely distributed in brain (Anderson et al., 1996). Othersources that may contribute to elevated extracellular adenosinelevels include release via Na⁺-independent transporters and release of ATP followed by enzymaticdephosphorylation to adenosine.

In summary, we have demonstrated that by disrupting transmembrane Na⁺ gradients, reversal of Na⁺-dependent nucleoside transporters can mediate cellular releaseof nucleosides. The evidence that this release is transporter-mediatedincludes inhibition by transport inhibitors and stimulation bytransporter permeants. Adenosine, a nucleoside with diverse receptor-mediatedeffects, may be released from cells by this process during conditions,such as ischemia, that depress cellular transmembrane Na⁺ gradients by compromising intracellular ATP levels and/or Na⁺/K⁺ ATPase function.

	Acknowledgments

We would like to thank Dr. J.D. Geiger, Dr. R. Bose, Ms. Wei Xiong, Mr. Kallol Mukherjee, Ms. Suzanne Delaney and Ms. IreneFoga for technical assistance.

	Footnotes

Accepted for publication December 16, 1996.

Received for publication August 26, 1996.

¹ This work was supported by the Medical Research Council of Canada (MRCC). F.E.P. is a Scholar of the MRCC.

Send reprint requests to: Dr. F.E. Parkinson, Department of Pharmacology and Therapeutics, University of Manitoba, 770 Bannatyne Avenue, Winnipeg, Canada R3E 0W3.

	Abbreviations

NBMPR, nitrobenzylthioinosine or nitrobenzylmercaptopurine riboside.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

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