From the Renal Division, Department of Medicine,
Physiology & Biophysics, Albert Einstein College of Medicine,
Bronx, New York 10461 and the § Division of Nephrology and
Hypertension, Department of Medicine, University of California, San
Diego, Veterans Affairs Medical Center,
San Diego, California 92093
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ABSTRACT |
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We recently identified a novel prostaglandin
transporter called PGT (Kanai, N., Lu, R., Satriano, J. A., Bao,
Y., Wolkoff, A. W., and Schuster, V. L. (1995)
Science 268, 866-869). Based on initial functional
studies, we have hypothesized that PGT might mediate the release of
newly synthesized prostaglandins (PG), epithelial transport of PGs, or
metabolic clearance of PGs. Here we examined the mechanism of PGT
transport as expressed in HeLa cells and Xenopus oocytes,
using isotopic PG influx and efflux studies. In both native HeLa cells
and oocytes, cell membranes were poorly permeable to PGs. In contrast,
in oocytes injected with PGT mRNA, the PG influx permeability
coefficient was 90-157 times that of oocytes injected with water. The
rank order substrate profile was PGF2
PGE2 > TXB2
6 keto-PGF1
.
PG influx displayed an overshoot with rapid accumulation of tracer
PGE2, followed by a gradual return to baseline. Based on
estimated oocyte volumes, the PGT-mediated accumulation of
PGE2 reached steady state at intra-oocyte concentrations
25-fold higher than the external media. The accumulation of PG was not
due to intracellular binding or metabolism. PGT-mediated uptake was
ATP- and temperature-dependent, but not
sodium-dependent, and was inhibited by disulfonic
stilbenes, niflumic acid, and the thiol reactive anion MTSES
(Na(2-sulfonatoethyl)methanethiosulfonate). [3H]PGE2 efflux from PGT-transfected HeLa
cells was stimulated by external (trans) PGE2 in a
dose-dependent fashion and was inhibited by bromcresol
green and 4,4'-diisothiocyanatostilbene-2,2'-disulfonate. Membrane
depolarization inhibited uptake of [3H]PGE2,
consistent with a model of net outward movement of negative charge
during the translocation event. These findings suggest that PGT
mediates [3H]PGE2 accumulation via
obligatory, electrogenic anion exchange.
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INTRODUCTION |
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Prostaglandins (PGs)1
and thromboxanes have broad physiologic and pathophysiologic effects,
regulating cellular processes in nearly every tissue. They elicit
potent actions on the cardiovascular, gastrointestinal, respiratory and
reproductive systems, and are important mediators of inflammation,
fever, and pain (2). As autacoids, PGs are synthesized by intracellular
enzymes at or near their sites of action before they are presented to
adjacent PG receptors. Thereafter, extracellular PGs are metabolized
in situ within seconds before they are able to reach the
general circulation (3, 4). At least in the case of PGE2
and PGF2, loss of biologic activity is due to cellular
uptake followed by intracellular oxidation (5-8).
At physiologic pH, PGs predominate as the charged organic anion (9) and diffuse poorly through the lipid bilayer (10, 11). Facilitated, carrier-mediated PG transport has been demonstrated by many diverse tissues including the lung (8, 12), liver (13), kidney (14), vagina and uterus (15), and blood-brain and blood-intraocular fluid barriers (16).
The clearance and metabolism of PGs from the pulmonary circulation has
been widely studied using the isolated, perfused rat lung model where
concentrative uptake of PGs has been described followed by the
appearance of metabolites in the venous effluent (8, 17). Substances
that inhibit PG transport reduce PG inactivation by the lung (18).
Moreover, whereas PGE1, PGF2,
PGD2, and PGI2 are all good substrates for the
oxidizing enzyme 15-hydroxyprostaglandin dehydrogenase,
PGI2 escapes pulmonary metabolism (8). These phenomena are
best explained by selective, carrier-mediated PG transport.
Transepithelial PG transport has also been clearly demonstrated in several tissues. In the brain where PGs are ineffectively metabolized (19), accumulation of PGs in the extracellular fluids of the brain would be expected to have adverse effects. Transepithelial transport of PGs across the blood-brain barrier to sites of cellular uptake and metabolism would therefore be necessary for removal of locally released PGs. Indeed, saturable and inhibitable carrier-mediated transport of PG has been demonstrated in tissues of the blood-brain and blood-intraocular fluid barriers, as well as across the rabbit vagina (20, 21), and the renal proximal tubule (14).
It is less clear if a carrier-mediated process facilitates the release of intracellular PGs across the cell membrane. Newly synthesized PGs, localized in the cell cytosol (22), might exit from the cell via a permease or via diffusion through the plasma membrane. On the other hand, as PGs are synthesized on the luminal surface of the endoplasmic reticulum they may conceivably be released from the lumen of the ER via fusion with the plasma membrane in a sort of "secretory pathway."
Until recently, little has been known about PG transport at a molecular level. Our laboratory recently identified a broadly expressed PG transporter (PGT) (1). In the present study, the mechanisms of PG transport by PGT were investigated both in transfected HeLa cells and in PGT-expressing Xenopus laevis oocytes. Our results provide evidence for active, energy-dependent accumulation of PGs as the organic anion via an exchange mechanism.
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EXPERIMENTAL PROCEDURES |
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Materials
All salts were of analytic grade, and were purchased from Sigma.
Succinic acid, malic acid, glutamic acid, -ketoglutaric acid,
aspartic acid, fumaric acid, oxaloacetic acid, and lactic acid were
purchased from Sigma. The disulfonic stilbenes H2-DIDS and
DIDS were purchased from Pierce (Rockford, IL), niflumic acid was
purchased from Sigma, and MTSES
/MTSEA+ were
purchased from Toronto Research Chemicals Inc. (Ontario, Canada).
Tritiated PGs were from NEN Life Science Products Inc. (Boston, MA).
All chemicals were of the purest grade available.
Transient Expression in HeLa Cells
Full-length PGT cDNAs cloned in pGEM-3z with coding strand downstream of the T7 promoter were transfected into HeLa cells. Cells grown to 80% confluence on 35-mm dishes were infected with recombinant vaccinia virus vTF7-3 (23) for 30 min and then transfected by adding PGT cDNA (10 µg/ml) and Lipofectin (20 µl/ml, Life Technologies, Inc., Gaithersburg, MD). Transfection with the plasmid pBluescript was used as a negative control. After 3 h of incubation, the medium was changed (Dulbecco's modified Eagle medium plus 5% fetal bovine serum, 100 units/ml penicillin/streptomycin) and the cells were maintained overnight in humidified incubators with 5% CO2 at 37 °C. Isotopic influx and efflux experiments were performed 18-22 h after transfection.
Transport Measurements in HeLa Cells
Influx Measurements--
The cell monolayers were washed twice
with a balanced salt solution (BSS) (135 mM NaCl, 13 mM H-Hepes, 13 mM Na-Hepes, 2.5 mM
CaCl2, 1.2 mM MgCl2, 0.8 mM MgSO4, 5 mM KCl, and 28 mM D-glucose). Influx measurements were
initiated by the addition of tritiated PGE2 (NEN Life
Science Products Inc.) to the flux media (BSS) to reach a final
concentration of <1.5 nM, which is well below the
Michaelis constant (Km) for PGT (1). Influx
measurements were carried out at room temperature over 10 min to 2 h. Isotopic influx experiments were terminated by aspiration of the
incubation media followed by two rapid washings with ice-cold 5%
bovine serum albumin in BSS and two additional washings with ice-cold
BSS. The cells were scraped into 1 ml of saline, mixed with liquid scintillation mixture (National Diagnostics, Atlanta, GA), and analyzed
by liquid scintillation counting. Influx values in all experiments were
calculated as femtomoles per mg of protein per nanomolar concentration
[3H]PGE2 and expressed as means ± S.E.
from duplicate monolayers. In some experiments, uptake studies were
performed in the presence of unlabeled substrates (succinic acid, malic
acid, glutamic acid, -ketoglutaric acid, aspartic acid, fumaric
acid, oxaloacetic acid, and lactic acid).
Efflux Measurements-- HeLa cell monolayers were preloaded with isotopic PGE2 by incubation with [3H]PGE2 for 20 min prior to efflux measurements. Immediately after incubation, cells were washed twice with room temperature BSS to remove adherent [3H]PGE2. At time 0, 1 ml of BSS was added to each monolayer. At each subsequent time interval (2-40-min intervals in different experiments) the 1 ml of efflux media was removed for scintillation counting and 1 ml of fresh BSS was added. At the end of the experiment, the cell monolayers were scraped and analyzed by scintillation counting. The remaining counts/min in the cells was added to the sum of the effluxed counts to estimate the amount of isotope loaded. Efflux rate constants were calculated from curve fitting with an iterative method (Deltagraph, Monterey, CA) using a single-exponential. In separate experiments, efflux was measured in BSS with various concentrations of unlabeled PGE2, or in BSS with unlabeled PGE2 and 300 µM DIDS or 50 µM bromcresol green (BCG). DIDS and BCG were added for 2 min before unlabeled PGE2.
Oocyte Preparation and mRNA Injection
Mature female X. laevis frogs (Xenopus I, Ann Arbor, MI) were anesthetized by hypothermia and 0.4% topical tricane. Ovarian tissue was removed via a 1-cm flank incision, then minced and placed in 2 mg/ml collagenase A (Boehringer Mannheim, Indianapolis, IN) for 1-2 h at 20 °C with gentle continuous agitation to remove the follicular layer. The oocytes were then washed with ND96 (96 mM NaCl, 2 mM KCl, 1 mM MgCl2, 5 mM Hepes, 1.8 mM CaCl2, pH 7.5). Mature oocytes (stage IV-V) were separated and stored in ND96E (ND96 plus 2.5 mM pyruvate, 0.5 mM sodium phosphate, and 100 units/ml penicillin/streptomycin) at 18 °C overnight prior to injection. mRNA was prepared using the mRNA capping kit (Stratagene, La Jolla, CA) by linearizing plasmids encoding PGT with XbaI and transcribing capped RNA using T7 RNA polymerase. 30 ng of mRNA in 50 nl of water were injected into individual oocytes using a microinjection apparatus. 50 nl of water were injected into oocytes as a control. Injected oocytes were incubated in ND96E for 2-3 days prior to isotopic PG influx and efflux studies. The incubation medium was changed daily.
Transport Measurements in Xenopus Oocytes
Influx Measurements--
Preliminary experiments indicated that
tracer PG uptake was the same in ND96 and BSS; accordingly, all fluxes
were determined in the latter medium. In some cases sodium chloride was
substituted with either choline chloride or lithium chloride. Tritiated
prostaglandins were added to the flux media to reach a final
concentration of 0.2-1.7 nM. A preliminary time course of
PGT-mediated [3H]PGE2 uptake was performed
over 3 h at room temperature. Subsequent influx experiments were
performed over 30 min, during which PG uptake was linear with time.
Groups of 10-15 oocytes were placed in micro-Eppendorf tubes
containing 500 µl of the appropriate influx media and isotopic PG.
Isotopic influx was terminated by removal of the flux media, followed
by rapid transfer through two 1-ml washes of ice-cold 5% bovine serum
albumin in BSS, followed by 2 additional washes of BSS. At the end of
the transport assay, a 100-µl aliquot of the flux media was measured
by scintillation counting. Individual oocytes were transferred to 10-ml
scintillation vials containing 500 µl of 10% SDS, scintillation
fluid was added, and the oocytes were counted. All influx values were
calculated as femtomoles per oocyte per nanomolar concentration of
substrate and expressed as means ± S.E. The intracellular
concentration of isotopic PG was calculated from the measured
counts/min in an estimated oocyte aqueous volume of 450 nl (24). All
oocytes from a single experiment were obtained from the same frog. In some experiments, influx measurements were determined in the presence of inhibitors of organic anion transport (disulfonic stilbenes or
niflumic acid), the water-soluble, thiol reactive anion
MTSES, or its cationic version MTSEA+.
Inhibitors were preincubated with oocytes prior to the start of the
transport assay and/or introduced with isotope where indicated. Some
oocytes were voltage clamped by the addition of 100 mM KCl prior to the influx assay. The cell membrane potential was determined in oocytes in BSS or high [K] using standard microelectrode
techniques. For trans-stimulation experiments, uptake assays were
performed on oocytes immediately after injection with unlabeled
PGE2 or candidate substrates (
-ketoglutaric acid,
succinic acid, glutamic acid, aspartic acid, and lactic acid).
Efflux Measurements-- Individual oocytes from a group in which PGT expression had been confirmed by tracer uptake were injected with 50 nl of BSS containing [3H]PGE2. Immediately after injection, an individual oocyte was placed in a 1.5-ml micro-Eppendorf tube containing 200 µl of BSS with or without unlabeled PGE2. At each subsequent 10-min time interval, 190 µl of efflux media was removed for scintillation counting and 190 µl of fresh efflux media was replaced. At the end of the experiment, the oocyte was lysed with 10% SDS (25). The counts/min in the lysed oocyte was added to the sum of the effluxed counts to estimate the amount of isotope injected. The data were plotted as % cpm remaining versus time. Curve fitting was performed as described previously.
PG Binding
Intracellular binding of PG was determined by three methods. First, oocytes and HeLa cell monolayers were preincubated in 0.015% Triton X-100 (26) prior to incubation with BSS containing [3H]PGE2. The degree of intracellular PG binding was determined by the increase in cell associated [3H]PGE2 in intact versus permeabilized cells. Second, oocytes were homogenized in a micro-Eppendorf tube using a pestle and the cell contents mixed in 1 ml of BSS media containing [3H]PGE2 in concentrations similar to those used in the transport assays (approximately 1 nM). The mixture (100-200 µl) was dialyzed against BSS (80 ml) using the Microdialyzer System 500 (Pierce) in the static mode. Prior to initiation of dialysis and at hourly intervals, 25-50 µl were removed from a sample well and counted. Third, PGT-expressing oocytes were subjected to the usual [3H]PGE2 influx, washed, and mechanically lysed in BSS. The accumulated [3H]PGE2 was dialyzed as described above to determine the degree of intracellular binding.
Metabolic Breakdown of Intracellular PGE2
To determine if the isotopic counts accumulated in PGT-expressing oocytes represented native PGE2 or metabolites, PGT-expressing oocytes were subjected to a 30-min [3H]PGE2 uptake assay and washed as described previously. The oocytes were then extracted in 100% methanol, centrifuged in methanol at 14,000 × g for 10 min, and the supernatant stored on dry ice for HPLC analysis. HPLC analysis with radiomatic detection was performed using a Phenomenex Ultramex C-18 column. The mobile phase was: A, H2O, 0.05% acetic acid with pH adjusted to 5.5 with ammonium hydroxide, and B, methanol:acetonitrile (1:1) at an initial composition of 10% B followed by a linear gradient to 55% B in 45 min and a second linear gradient to 100% B in the next 10 min at a flow rate of 0.2 ml/min. A sample of the initial isotopic influx media was used as a control.
Permeability Measurements
The PG permeability of PGT-injected oocytes compared with
water-injected oocytes was determined from the kinetics of isotopic PG
influx and efflux. The PG permeability coefficient P
(cm·s1) was calculated from the relation Jsolute
(mol·s
1) = P (cm·s
1)·SA
(cm2)·
concentration (moles·cm
3),
where J is the solute flux, SA is the oocyte surface area (0.045 cm2) assuming a smooth oocyte surface (24), and
concentration is the difference in solute concentration between inside
and outside the oocyte. In the influx experiments, we assumed that
concentration was the PG concentration in the influx media (no
intracellular PG at the initiation of the assay). In the efflux
experiments, we took
concentration as the concentration of
intracellular PG, calculated from the mean intracellular isotopic PG
during the efflux period.
Inhibitory Constants
Inhibitors were added at various concentrations during [3H]PGE2 uptake. K1/2 was determined by relating the uninhibited uptake rate to the inhibited uptake rate calculated from the relation,
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(Eq. 1) |
Effect of ATP Depletion on PGT-mediated Influx
Some PGT-expressing oocytes were incubated in 3 mM iodoacetic acid in N2 equilibrated BSS for 3 h prior to the transport assay. As a control, oocytes from the same group were incubated in standard air-equilibrated BSS without iodoacetate. The intracellular ATP concentration was also measured in similarly treated oocytes using an ATP assay (Sigma) based on the enzymatic reaction described by Bucher (28).
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RESULTS |
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PG Permeability of Native Plasma Membranes Is Low-- It has been previously reported that PGs at physiologic pH diffuse poorly across lipid bilayers. Here we determined the permeability coefficients (P), calculated from the means of the solute fluxes, for 10-min PGE2 influx and efflux in native Xenopus oocytes (Table I). Efflux coefficients were obtained by measuring the amount of [3H]PGE2 release into the external media over the first 10 min following injection of [3H]PGE2. As shown in Fig. 1, this 10-min efflux was linear over intraoocyte concentrations from 35 to 380 nM [3H]PGE2, suggesting simple diffusion across the lipid bilayer. The permeability coefficient for efflux is the same as for influx, indicating that PG entry and exit from native Xenopus oocytes occurs by simple diffusion. Permeability coefficients for mannitol and para-aminohippurate (data not shown) were in agreement with those published by others (29, 30), indicating that our oocytes are comparable to those reported in the literature.
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PGT Mediates Concentrative PG Uptake in HeLa Cells and Xenopus
Oocytes--
We previously reported that transient PGT expression in
HeLa cell monolayers resulted in PG influxes with a clear rank order for various PG substrates (31). Here we established the
Xenopus oocyte as a PGT expression system as follows.
PGT-mediated [3H]PGE2 influx in oocytes
increased as a function of the amount of injected mRNA (0-25
ng/oocyte) and peaked 3-5 days after injection (data not shown). PGT
caused significant increases in tritiated PG influx when compared with
water-injected oocytes with the following rank order profile:
PGF2
PGE2 > TXB2
6-keto-PGF1
. This is similar to the rank order of PGT
expressed in mammalian cells (1). In PGT-expressing oocytes, the
permeability coefficients for PGF2
, TXB2,
and PGE2 were increased 157-, 90-, and 49-fold, respectively, over that of water-injected oocytes. For
6-keto-PGF1
and AA, the PGT-associated increase in
permeability was only 7- and 1.5-fold, respectively, that of
water-injected oocytes (Table II).
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PGT Transport Is Energy-dependent-- To test further the hypothesis that PGT-mediated uptake is active, we examined the degree to which transport is sodium dependent. PGT-expressing oocytes were preincubated in either BSS or sodium-free BSS (substituted with either 140 mM choline or 140 mM lithium) for 2.5 h prior to a 30-min uptake assay. Uptake was then conducted either with or without extracellular sodium. Tracer uptake was not significantly changed in choline substituted media (3.7 ± 0.2 fmol/oocyte), or lithium substituted media (2.8 ± 0.3 fmol/oocyte) as compared with media containing sodium (3.2 ± 0.3 fmol/oocyte).
We tested the effect of ATP depletion on [3H]PGE2 uptake by incubating PGT-expressing oocytes in either 3 mM iodoacetic acid under nitrogen gas or in BSS as a control for 3 h prior to the uptake assay. As shown in Fig. 6, there was a 63 ± 8% decrease in PGT-mediated uptake in ATP-depleted oocytes compared with controls (2.5 ± 0.3 fmol/oocyte versus 6.8 ± 0.7 fmol/oocyte). The intracellular ATP concentration of control oocytes (n = 50) averaged 360 ± 65 µmol/dl, as compared with 50 ± 65 µmol/dl in oocytes (n = 50) preincubated with 3 mM iodoacetate (73 ± 19% decrease concentration). Thus, PGT-mediated uptake varies with intracellular ATP concentration. Uptake under ice-cold conditions was also decreased by 85 ± 4% compared with uptake performed at room temperature (1 ± 0.2 fmol/oocyte versus 6.8 ± 0.7 fmol/oocyte).
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PGT Mediates [3H]PGE2 Transport via Anion
Exchange--
To determine whether PGT translocates its substrate as
the neutral or the charged species, PGT-mediated
[3H]PGE2 influx was examined in the presence
of the classic anion transport inhibitors, the disulfonic stilbenes, as
shown in Fig. 7. Groups of PGT-expressing
and water-injected oocytes were preincubated with either BSS as a
control or in varying amounts of H2-DIDS or DIDS (100 µM to 5 mM) for 15 min before the tracer
uptake. The addition of DIDS and H2-DIDS produced
substantial inhibition of tracer PGE2 uptake with
inhibitory constants (K1/2) of 23 and 29 µM, respectively. Incubation of PGT- expressing oocytes
for 15 min with DIDS or H2-DIDS, followed by washing,
restored subsequent tracer PGE2 uptake to 80 and 65% of
normal indicating reversibility (data not shown). In contrast,
incubation for 40 min followed by washing, produced irreversible
inhibition (DIDS, 0.6 ± 0.1 fmol/oocyte; and H2-DIDS,
0.3 ± 0.03 fmol/oocyte versus control, 1.5 ± 0.5 fmol/oocyte) indicating covalent blockade. Another anion transport
inhibitor, niflumic acid, also inhibited uptake with an estimated
K1/2 of 150 µM (data not shown). In
other experiments, PGT-expressing oocytes were preincubated in media
containing either the small, thiol reactive anion MTSES
or its cationic version MTSEA+ for 10 min prior to the
transport assay and then washed. As shown in Fig.
8, MTSES
pretreatment
caused a dose-dependent reduction in subsequent [3H]PGE2 uptake. This effect was reversible
by co-incubation in dithiothreitol (data not shown). On the other hand,
pretreatment with the cationic version of the compound,
MTSEA+, had no effect on uptake. The data support a
permeation model in which the substrate binding region of PGT contains
fixed positive charges to concentrate anionic substrate within the pore
to increase translocation. If the surface charges in the substrate
translocation pathway are made more negative, i.e. by the
introduction of MTSES
, then the concentration of anionic
substrate within the pore pathway is reduced, leading to a decrease in
transport.
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DISCUSSION |
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We functionally characterized transport properties of the prostaglandin transporter "PGT" as expressed in HeLa cells and X. laevis oocytes using labeled PGE2 as substrate. In the present work, we have established the oocyte as a PGT expression system by demonstrating significant increases in labeled PG influx in PGT-expressing oocytes with the same substrate profile as that previously described in transfected HeLa cells. The baseline influx and efflux permeabilities for tracer PGE2 in control oocytes were very low (Table I). In contrast, PGT expression increased the permeability coefficient for influx of tracer PGE2 by approximately 50-fold (Table II). The [3H]PGE2 uptake in both PGT-transfected HeLa cells and PGT-expressing oocytes displayed an overshoot characterized by time-dependent, saturable accumulation of substrate, followed by a gradual return to baseline (Fig. 2). Calculation of the transmembrane gradient at peak accumulation of [3H]PGE2 minus intracellular binding of [3H]PGE2, as estimated from oocyte volumes, demonstrated 20-fold concentrative uptake of PGE2 relative to the external medium.
Accumulation of isotope could be misinterpreted as uphill transport of substrate if there were substantial intracellular binding. In this case, the cytosolic concentration of tracer PG just inside the plasma membrane would be maintained at a low level by continual off-loading onto the binding site, driving passive diffusion. Our data offer two compelling arguments against this possibility. First, using dialysis methods we took pains to identify PG binding capacity in the cytosol of oocytes, but found that this was negligible. Second, the response to detergent is in the wrong direction. If the plasma membrane represents a rate-limiting barrier in the access of PG to a significant intracellular binding site, then increasing the passive membrane permeability by a light detergent treatment should greatly increase oocyte-associated tracer counts. Instead, we found that counts decreased in the permeabilized oocyte (Fig. 3). These results are not consistent with a binding sink, but rather suggest an active uptake model in which the detergent has introduced a route for the back-leak of tracer PG out of the cell.
Intracellular metabolism represents another mechanism by which a PG uniporter could be misinterpreted as causing uphill transport of tracer. In this scheme, PGE2 would be metabolized inside the oocyte, thus maintaining the inwardly-directed gradient for native PGE2. We showed, however, that there is essentially no metabolism of tracer PGE2 inside the oocyte (Fig. 5), thus excluding this possibility.
Our data clearly indicate concentrative PG uptake. We have demonstrated that PG uptake varies with intracellular ATP, in that reduction of intracellular ATP levels by 73% was associated with a reduction in PGT-mediated PG uptake of 63% (Fig. 6). Analysis of the deduced amino acid sequence of PGT demonstrates no ATP binding motifs or homology to P-type ATPases. Rather, PGT shares a common structural motif with members of the "major facilitator superfamily" (35). Hence, ATP is probably indirectly involved in PG transport.
Experiments in the present series exclude sodium-dependent PG uptake. These results confirm our previously published data using HeLa cells. In addition, our earlier studies showed that PGT-mediated uptake is neither Cl- nor H+-dependent (1).
PGT-mediated uptake exhibits an "overshoot," which is consistent with uptake coupled to the counterflow of a substrate down its concentration gradient, which is dissipated over time. Either a uniporter or antiporter can demonstrate this phenomenon. In the case of a uniporter, movement of substrate down its concentration gradient can occur in the absence of a trans-substrate. However, we observed no PGT-mediated transport in the absence of trans-PGE2, and there was no inhibition by BCG or DIDS under these conditions (Fig. 9, A and D). In contrast, there was a 4-5-fold increase in tracer PGE2 efflux in PGT-expressing cells in the presence of external PGE2. Isotopic efflux experiments into varying concentrations of extracellular PGE2 displayed an apparent Km for extracellular PGE2 similar to that measured by cis-inhibition (290 nM) (31). Furthermore, inhibitors of PGT-mediated uptake (Fig. 9C) also inhibited trans-stimulated efflux. This clear trans-dependence suggests that PGT functions as an obligate exchanger.
Several classic anion transport inhibitors, including the stilbene
disulfonates and niflumic acid, block PGT-mediated PG uptake (Fig. 7).
In addition, introduction of the small, water-soluble, anionic,
thiol-reactive agent MTSES blocks transport, whereas its
cationic version (MTSEA+) does not (Fig. 8). Inhibition of
transport by MTSES
by not MTSEA+ argues for
the presence of fixed positive charges in the substrate translocation
pathway. Other evidence from our laboratory also strongly argues for
transport of the anion. First, site-directed mutagenesis of two
conserved cationic amino acids (Arg-560 and Lys-613) in rat PGT
abolishes transport,2
suggesting that these residues play an important electrostatic role in
substrate translocation. Second, removal of the 1-position carboxyl
charge abolishes substrate affinity (31).
To begin to test whether PGT-mediated anion exchange is electrogenic or
electroneutral, we analyzed the effect of membrane depolarization on PG
uptake. In the presence of high external [K] or [BaCl2]
to depolarize the membrane potential, PG transport is decreased.
Furthermore, the fall in [3H]PGE2 uptake with
high external [K] (3.2-fold) is similar to the change in the
electrical driving force for a monovalent anion from a membrane
potential of 43 to
17 mV (2.8-fold). This concordance is consistent
with electrogenic anion exchange in which there is a net transfer of
one negative charge out for each PG anion taken up.
Taken together, the data suggest that PGT-mediated influx of PGs may be
coupled to the efflux of a counter-anion resulting in an net outward
movement of negative charge. This counter-anion (substrate "X")
might be present at a high intracellular concentration and may be
reduced by ATP depletion. An example is the exchange driven uptake of
p-aminohippurate by -ketoglutarate in the basolateral membrane of the renal proximal tubule. In this regard, we tested several divalent Kreb cycle intermediaries as candidates for substrate X. Unfortunately, we were unable to identify any that caused
cis-inhibition of tracer PGE2 uptake in PGT-expressing HeLa
cells, or trans-stimulation of PGE2 uptake.
Understanding the molecular mechanism of PGT transport may lead to
insights into the molecular biology of other organic anion transporter
proteins. The deduced amino acid sequence of rat PGT has 37% identity
with a rat organic acid transporter called "oatp" (36), and 35%
identity with the recently identified rat organic anion transporter
called OAT-K1 (37). Although all three organic anion transporters have
distinct substrate specificities (oatp transports charged steroids;
OAT-K1 transports methotrexate), their deduced primary and putative
secondary structure indicate that they are members of a family of
organic anion transporters sharing a common mechanism. In the case of
oatp and PGT, depletion of ATP led to a reduction in function. On the
other hand, maneuvers to deplete ATP in OAT-K1 had no effect on
function; however, ATP levels were not measured in the treated cells.
Transport by all three transporters has been found to be
sodium-independent. Substrate accumulation by OAT-K1 was unaffected by
imposed Cl and H+ gradients (37) whereas
preliminary experiments with oatp suggest possible exchange-driven
transport with HCO3
. Understanding the
precise transport mechanisms of each of these transporters awaits
further investigation.
What is the purpose of PG uptake for the organism? As discussed in the Introduction, carrier-mediated concentrative PG transport has been described in a variety of tissues, where it is felt to play a role in the metabolic clearance of PGs. Carrier-mediated PG removal appears necessary, since the plasma membrane appears to have a low intrinsic permeability to PGs. Indeed, our data demonstrate that the plasma membranes of control oocytes have a very low baseline PG influx permeability coefficient for several different PGs (Table I), a finding that is in agreement with previous results obtained by Bito and Baroody (10) using the erythrocyte as a model membrane, as well as with our recently published data using HeLa cells (31).
Eling and co-workers carried out an impressive analysis of the structural requirements needed for PGs to undergo metabolic clearance by the isolated, perfused rat lung (38). Our laboratory recently published the substrate structural requirements of PGT (31). A comparison of the two studies indicates that metabolic PG clearance by the rat lung and PG transport by PGT are virtually indistinguishable with regard to the structural requirements of the substrate molecule. Moreover, if inhibitors of PG transport are introduced into the perfused rat lung, there is decreased PG metabolism, as demonstrated by a decrease in the concentrations of the inactive oxidized derivatives and an increase in the concentration of the biologically active PG in the venous effluent (8, 17). Interestingly, the inhibitor profile and Ki values found for the perfused rat lung and for PGT are similar (bromcresol green, 2-4 µM; indocyanine green, 16 µM; furosemide, 25-80 µM) (1). Furthermore, there is evidence that this uptake of prostanoids is concentrative and independent of Na+-K+-ATPase activity (13, 20, 32). Thus, taken together with the present study our data strongly indicate that PGT most likely mediates the removal of PGs in the lung prior to their intracellular oxidation (6, 39, 40).
The exact route by which newly synthesized endogenous PGs are released from cells remains uncertain. Cyclooxygenase types I and II have been localized to the endoplasmic reticulum, and modeling and immunological data suggest that the active sites face the endoplasmic reticulum lumen. Moreover, when fluorescent cyclooxygenase substrates are introduced into the cytosol, they appear to be activated there (22). Thus, the standard paradigm is that newly synthesized PGs appear in the cytosol. If this were the case, then PGs would need to subsequently traverse the plasma membrane, either by simple diffusion or by a carrier-mediated mechanism (e.g. PGT). We have shown that PGs may exit the cell by simple diffusion (Fig. 1); however, it is unclear whether this slow rate of diffusion is sufficient to mediate PG release from cells. Preliminary data from our laboratory have localized PGT to renal cells that are known to release PGs, i.e. interstitial cells and collecting duct cells,3 suggesting that PGT may play a role in PG release. Moreover, since we have shown that PGT can mediate both influx and efflux of PGs, it is possible that PGT may mediate PG release in specific cell types. An example of such a bidirectional transporter is erythrocyte band 3 ("AE1") which mediates bicarbonate uptake into erythrocytes in the pulmonary circulation, but bicarbonate release from erythrocytes in the periphery.
In summary, the present studies confirm, and significantly extend, our initial report on PGT as a novel prostaglandin transporter. In the present study, we have demonstrated PGT-mediated accumulation of PGs via a mechanism that is consistent with obligatory, electrogenic anion exchange. The current model suggests that PGT may be involved with metabolic clearance and/or PG release from cells.
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ACKNOWLEDGEMENTS |
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We thank Vyto Versalis for membrane potential measurements and Robert Murphy for HPLC analyses.
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FOOTNOTES |
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* This work was supported by National Institute of Diabetes and Digestive and Kidney Diseases Grants RO1-DK49688, KO8-DK02492, and DK07110.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
¶ To whom correspondence should be addressed: Renal Division, Ullman 615, 1300 Morris Park Ave., Bronx, NY 10461. Tel.: 718-430-3158; Fax: 718-430-8963; E-mail: schuster{at}aecom.yu.edu.
1 The abbreviations used are: PG, prostaglandin; DIDS, 4,4'-diisothiocyanatostilbene-2,2'-disulfonate; H2-DIDS, 4,4'-diisothiocyanatodihydrostilbene-2,2'-disulfonate; BCG, bromcresol green; MTSES, Na(2-sulfonatoethyl)methanethiosulfonate; MTSEA, MTS-ethylammonium; BSS, balanced salt solution; HPLC, high performance liquid chromatography.
2 B. Chan and V. L. Schuster, unpublished observations.
3 Y. Bao and V. L. Schuster, unpublished observations.
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