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1 Physiologisches Institut und 2 Zentrum für Innere Medizin, Abteilung für Kardiologie, Justus-Liebig-Universität, D-35392 Giessen, Germany
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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We investigated the relationship between the
ATP-evoked rise of cytosolic Ca2+
concentration
([Ca2+]i)
and barrier function in porcine aortic endothelial monolayers. ATP
(0.01-100 µM) induced a transient rise of
[Ca2+]i
and reduced permeability in a concentration-dependent manner. In
contrast, the Ca2+ ionophore
ionomycin (1 µM) elicited a rise in
[Ca2+]i
comparable to that induced by ATP (10 µM), but it increased permeability. For the reduction of permeability, nucleotides were found
to be in the following order of potency: ATP = ATP
S > ADP = UTP.
Blockade of adenosine receptors by 8-phenyltheophylline (10 µM) did
not affect ATP (10 µM)-induced reduction of permeability. ATP reduced
permeability even in endothelial monolayers that had been loaded with
the Ca2+ chelator BAPTA to prevent
the rise in
[Ca2+]i.
U-73122 (1 µM), an inhibitor of phospholipase C (PLC), completely abolished the effect of ATP (10 µM) on permeability. It also
abolished the translocation of protein kinase C (PKC) in response to
ATP, which could also be achieved by the PKC inhibitors Gö-6976
(100 nM) or bisindolylmaleimide I (1 µM). In the presence of PKC
inhibitors, however, the permeability effect of ATP was not affected.
The presence of inhibitors of adenylate or guanylate cyclase (50 µM SQ-22536 or 20 µM ODQ) prevented changes in cyclic nucleotides but
did not affect the permeability effects of ATP. The study shows that
ATP reduces macromolecule permeability via a PLC-mediated mechanism
that is independent of the concomitant effects of ATP on cytosolic
Ca2+, cyclic nucleotides, or PKC.
adenosine 5'-triphosphate; paracellular permeability; phospholipase C; protein kinase C; cyclic nucleotides
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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ATP IS AN IMPORTANT MEDIATOR involved in signaling between cardiovascular cells. Extracellular levels of ATP are normally maintained at extremely low levels due to ubiquitous ectonucleotidases, which rapidly hydrolyze nucleotides. However, in the vasculature significant amounts of extracellular ATP may locally accumulate at the site of thrombus formation (6) due to a release from activated platelets or in the hypoxic myocardium (4) when ATP is released together with degradation products such as adenosine from energy-depleting myocardial cells. A systemic increase in ATP and its immediate hydrolytic products up to micromolar concentrations is found in blood plasma under conditions of traumatic shock (9).
ATP may act on endothelial cells through multiple receptors and second messengers. The majority of known effects elicited by nonhydrolyzed ATP are mediated via P2y and P2u receptors (5). These receptors are both coupled to phospholipase C (PLC), but via distinct G proteins (21). Signal transduction events stimulated by ATP include the inositol lipid-Ca2+ signaling cascade, protein kinase C (PKC), and, directly or indirectly, activation of soluble guanylate cyclase or adenylate cyclase (6). ATP may also act on endothelial cells after degradation to adenosine via adenosine receptors (25).
The information on ATP effects on endothelial barrier function is scarce and inconsistent. Depending on the endothelial cell population, ATP can modulate endothelial barrier function in one direction or the other. In the special case of microvascular endothelium contained in venular microvessels from frogs (13-16), ATP was found to increase paracellular permeability. Similar to effects of inflammatory mediators, this rise of permeability in response to ATP coincided with a rise in cytosolic Ca2+ concentration ([Ca2+]i) within the cells. In other populations, ATP was found to decrease paracellular permeability. Examples are bovine aortic endothelial cells (12) or, from preliminary experiments of the present study, cultured endothelial cells from other macrovessels such as the porcine aorta, porcine pulmonary artery, bovine aorta, or human umbilical vein. In this second type of reaction, the role of [Ca2+]i is unclear. The present study was undertaken to analyze the role of [Ca2+]i changes in endothelial cell preparations in which ATP reduces permeability. The effects of ATP were contrasted with those of ionomycin, a Ca2+ ionophore, which causes a rise in [Ca2+]i in a receptor-independent manner. Endothelial barrier function was studied by determining the passage of albumin through confluent monolayers of porcine aortic endothelial cells. Variations of albumin passage in this model are to be attributed to changes in paracellular permeability.
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Cell cultures. Endothelial cells from the bovine aorta, porcine aorta, and pulmonary artery were isolated and cultured as previously described (26). Human endothelial cells from umbilical cords were isolated and cultured according to van Hinsberg et al. (30). Confluent cultures of primary endothelial cell were trypsinized in phosphate-buffered saline [PBS; composed of (in mM) 137 NaCl, 2.7 KCl, 1.5 KH2PO4, and 8.0 Na2HPO4, pH 7.4, supplemented with 0.05% (wt/vol) trypsin and 0.02% (wt/vol) EDTA] and seeded at a density of 7 × 104 cells/cm2 on 24-mm round polycarbonate filters (pore size 0.4 µm), 5 × 20-mm glass coverslips, or 30-mm culture dishes for determination of albumin permeability, [Ca2+]i, or cyclic nucleotide contents, respectively. Experiments were performed with confluent monolayers 4 days after seeding.
Macromolecule permeability. The permeability of the endothelial cell monolayer was studied in a system of two compartments separated by a filter membrane (23, 24). Both compartments contained as basal medium modified Tyrode solution [composition in mM: 150 NaCl, 2.7 KCl, 1.2 KH2PO4, 1.2 MgSO4, 1.0 CaCl2, and 30.0 N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid (HEPES); pH 7.4, 37°C] supplemented with 5% (vol/vol) heat-inactivated newborn calf serum (NCS; 10 min at 60°C). There was no hydrostatic pressure gradient between the compartments. The "luminal" compartment containing the monolayer had a volume of 2.5 ml, and the "abluminal" compartment had a volume of 13 ml. The fluid in the abluminal compartment was constantly stirred. Trypan blue-labeled albumin (60 µM) was added to the luminal compartment. The appearance of labeled albumin in the abluminal compartment was continuously monitored by pumping the liquid through a spectrophotometer (Specord 10; Zeiss, Jena, Germany). Increases in the concentration of labeled albumin were detected with a time delay of <15 s. The concentration of labeled albumin in the luminal compartment was determined every 10 min during incubation. It did not change significantly in the time frame of the experiments.
The albumin flux [F; expressed in mol/(s · cm2)] across the monolayer with the surface area (S) was determined from the rise of albumin concentration (d[A]2) during the time interval (dt) in the abluminal compartment (volume V) as follows
![<IT>F</IT> = (d[A]<SUB>2</SUB> /d<IT>t</IT> × V)/<IT>S</IT>](/content/vol276/issue6/fulltext/H1892/img001.gif)
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![<IT>P</IT> = <IT>F</IT>/([A]<SUB>1</SUB> − [A]<SUB>2</SUB>)](/content/vol276/issue6/fulltext/H1892/img002.gif)
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[A]2) remained
virtually unchanged in the course of the described experiments, the
relative changes in F correspond to
similar changes in P.
Experimental protocols.
The basal medium used in incubations was modified Tyrode solution
(composition as described in Macromolecule
permeability). Macromolecule permeability of the
endothelial monolayer, transferred to the incubation chamber, was
determined after an initial equilibration period of 20 min. The basal
albumin permeability of each monolayer-filter system was then
determined during another 20 min of incubation. Agents were added as
indicated in RESULTS, and the response
of albumin permeability was recorded for another 40-80
min. For the incubations under
Ca2+-free extracellular
conditions, a Ca2+-free basal
medium (composition in mM: 150 NaCl, 2.7 KCl, 1.2 KH2PO4,
1.2 MgSO4, 0.5 ethylene
glycol-bis(
-aminoethyl
ether)-N,N,N',N'-tetraacetic acid (EGTA), and 30.0 HEPES; pH 7.4, 37°C) supplemented with
heat-inactivated 5% (vol/vol) NCS was used. Stock solutions of
bisindolylmaleimide I (BIM), Gö-6976, ionomycin,
1H-[1,2,4]oxadioazolo[4,3-a]quinoxalin-1-one (ODQ), SQ-22536, U-37122, U-37343, and thapsigargin were prepared with
dimethyl sulfoxide (DMSO). A stock solution of
1-O-octadecyl-2-O-methyl-rac-glycero-3-phosphorylcholine (ET-18-OCH3) was prepared with
absolute ethanol. Appropriate volumes of these solutions were added to
the cells, yielding final solvent concentrations 
0.1% (vol/vol). The
same final concentrations of DMSO or ethanol were also included in all
respective control experiments. Stock solutions of all other substances
were prepared in basal medium (composition as described in
Macromolecule permeability). Appropriate volumes of these solutions were added to the cells. Identical additions of basal medium were included in all respective control experiments.
Cytosolic Ca2+. Free [Ca2+]i were determined using the fluorescent Ca2+ indicator fura 2. Confluent endothelial monolayers cultured on 5 × 20-mm glass coverslips were incubated in medium 199 supplemented with 5% (vol/vol) heat-inactivated NCS and the addition of 5 µM fura 2-AM (acetoxymethyl ester of fura 2) at 20°C in the dark. After a 50-min incubation period, the extracellular fura 2-AM was removed by medium change. This was followed by a 20-min incubation period in the same medium before measurements were started. The coverslips were then aligned in a quartz cuvette into the beam of a fluorescence spectrophotometer (LS 50B; Perkin-Elmer, Überlingen, Germany). During incubations, the excitation wavelength was alternated between 340 and 380 nm (bandwidth 5 nm). Emitted light was detected at 510 nm (bandwidth 2 nm). Fura 2 fluorescence was calibrated according to the method described by Grynkiewicz et al. (10). For this purpose, the cells were exposed to 5 µM ionomycin in modified Tyrode solution containing either 3 mM Ca2+ or 5 mM EGTA to obtain the maximum (Rmax) and minimum (Rmin) of the ratio of fluorescence (R), respectively. [Ca2+]i was calculated according to the equation
![[Ca<SUP>2+</SUP>]<SUB>i</SUB> = <IT>K</IT><SUB>d</SUB> × &bgr; × (R − R<SUB>min</SUB>)/(R<SUB>max</SUB> − R)](/content/vol276/issue6/fulltext/H1892/img003.gif)
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is the ratio of the 380-nm
excitation signals of ionomycin-treated cells at 5 mM EGTA and 3 mM
Ca2+.
Loading of BAPTA-AM. Confluent endothelial monolayers cultured on either filter membranes or 5 × 20-mm glass coverslips were incubated in medium 199 supplemented with 5% (vol/vol) heat-inactivated NCS and the addition of 10 µM 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraacetic acid-AM (acetoxymethyl ester of BAPTA) at 37°C. After a 30-min incubation period, the extracellular BAPTA-AM was removed by medium change and the experiments were started.
Determination of PKC activity. The activity of PKC was determined in the membrane fraction of endothelial cells using the method of Chakravarthy et al. (3) that allows measurement of PKC activity in its native membrane-associated state. Cultured endothelial monolayers were incubated for the time indicated in RESULTS, and the cultures were then rinsed twice with ice-cold PBS and subsequently covered with ice-cold hypotonic lysis buffer (composition in mM: 1 NaHCO3, 5 MgCl2, and 0.1 PMSF; pH 7.4). The cells were scraped off the dish and vigorously mixed at room temperature for 2 min. The lysates were centrifuged at 1,000 g for 5 min at 4°C to sediment nonlysed cells and nuclei. The postnuclear supernatants were centrifuged at 4°C for 10 min at 425,000 g. The sedimented endothelial membranous fractions were resuspended in 200 µl of assay buffer (composition in mM: 0.002 CaCl2, 10 MgCl2, 0.2 PMSF, 2 NaF, 0.2 Na3P2O7, 0.2 Na3VO4, and 50 Tris · HCl buffer; pH 7.4).
The activity of PKC in the membrane fraction was determined by a continuous fluorescence assay using an acrylodan-labeled myristolated alanine-rich C kinase substrate (MARCKS) peptide (acrylodan-C-KKKKKRFSFKKSFKLSGFSFKKNKK) as PKC substrate (20). Fluorescence studies were performed at 22°C in the fluorescence spectrophotometer (LS 50B). The reaction mixture (total volume 0.7 ml) contained assay buffer, 10-50 µg protein of endothelial membrane fraction, and 75 nM acrylodan-labeled MARCKS-peptide. The reaction was started by 0.5 mM ATP. The fluorescence decrease during phosphorylation was monitored for 15 min at the 480-nm emission maximum of the acrylodan-labeled MARCKS peptide with excitation at 370 nm. PKC activity was determined from the initial slope of the fluorescence signal (fluorescence decrease per minute per 10 µg of membrane protein) and is expressed as the percentage of a defined control condition. To validate the continuous fluorescence assay, phosphate incorporation into the acrylodan-labeled MARCKS peptide was determined as described previously (22). Under defined control conditions, a decrease of fluorescence of 5.6 ± 0.9% per minute per 10 µg of membrane protein corresponded to a [32P]orthophosphate incorporation into the acrylodan-labeled MARCKS peptide of 580 ± 97 pmol · min
1 · 10 µg membrane protein1.
Cellular contents of cyclic nucleotides.
Cultured endothelial monolayers were incubated for the time indicated
in RESULTS. At the end of the
incubations, the incubation medium was aspirated, ice-cold ethanol was
added, and the culture dishes were stored at 80°C. To
determine the intracellular cyclic nucleotide contents, the ethanol was
evaporated at 60°C, and the samples were suspended in
double-distilled water, transferred into Eppendorf reaction tubes, and
centrifuged for 5 min at 14,000 g.
Cyclic nucleotide concentrations of the supernatants were determined by
using radioimmunoassays (Amersham, Braunschweig, Germany). The protein
contents of the samples were determined according to Bradford (1) using
bovine serum albumin as the standard.
Materials.
ODQ was from Alexis Biochemicals (Grünberg, Germany); Falcon
plastic tissue culture dishes were from Becton Dickinson (Heidelberg, Germany); acrylodan-labeled MARCKS peptide (as PKC fluorescence substrate), ATP, adenosine
5'-O-(3-thiotriphosphate)
(ATPS), ADP, AMP, and UTP were from Boehringer Mannheim (Mannheim,
Germany); BIM, ET-18-OCH3,
Gö-6976, ionomycin, SQ-22536, U-37122, U-37343, and thapsigargin
were from Calbiochem (Bad Soden, Germany); Transwell polycarbonate
filter inserts (24-mm diameter, 0.4-µm pore size) were from Costar
(Bodenheim, Germany); NCS, medium 199, penicillin-streptomycin, and
trypsin-EDTA were from GIBCO Life Technologies (Eggenstein, Germany);
and 5'-(N-ethylcarboxamido)adenosine (NECA) was from Sigma (Deisenhofen, Germany). All other chemicals were of the best
available quality, usually analytic grade.
Statistical analysis. Data are given as means ± SD of n = 6 experiments using independent cell preparations. Statistical analysis of data was performed according to Student's unpaired t-test. Probability (P) values of <0.05 were considered significant.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Macromolecule permeability.
Exposure of aortic endothelial monolayers to 10 µM ATP reduced their
albumin permeability from a control level of 5.8 ± 0.7 to 3.5 ± 0.9 × 106 cm/s after
20 min (Fig. 1). Albumin permeability
remained that low for a further 60 min. This observation was not
restricted to porcine aortic endothelial monolayers but was also made
in endothelial monolayers derived from the porcine pulmonary artery, bovine aorta, and human umbilical vein (Table
1). For the remainder of this study,
endothelial cells from the porcine aorta were used. In contrast to the
effect on permeability induced by ATP, the addition of ionomycin (1 µM) increased permeability rapidly to a peak value of 8.9 ± 0.5 × 106 cm/s within 10 min. Afterward, permeability decreased but remained significantly
elevated during the time of observation. The effects of ATP and
ionomycin on permeability were concentration dependent. Both agents
were tested in a concentration range between
108 and
105 µM (Fig.
2). The permeability experiments were
performed in the presence of 5% heat-inactivated NCS. This small
amount of serum was included in the incubation medium because basal
permeability of endothelial monolayers was then stable up to 2 h. Under
serum-free conditions, permeability was also reduced by 10 µM ATP
(from a control value of 6.7 ± 0.5 to 4.1 ± 0.5 × 106 cm/s after 20 min) or increased by 1 µM ionomycin (from a control value of 6.7 ± 0.5 to 9.7 ± 0.8 × 106 cm/s after 10 min).
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S reduced permeability to the
same extent as ATP. ADP as well as UTP also reduced albumin
permeability in a concentration-dependent manner, but these nucleotides
were less potent than ATP or ATPS. To test whether the ATP effect is
transmitted through adenosine receptors, endothelial cells were
preincubated for 10 min with 10 µM 8-phenyltheophylline (8-PT), an
inhibitor of adenosine receptors. As shown in Fig.
4, this pretreatment did not affect the
reduction of permeability induced by 10 µM ATP, but it significantly
inhibited the effect of 10 µM AMP or 100 nM NECA, a stable adenosine
analog, on albumin permeability.
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ATP-induced increase in
[Ca2+]i
and permeability.
Exposure of endothelial cells to 10 µM ATP, a concentration that
caused a marked reduction of albumin permeability, elicited a transient
rise of
[Ca2+]i
with a maximum of 503 ± 47 nM (Fig. 5).
The effect of ATP on [Ca2+]i
was comparable to that induced by 1 µM ionomycin. As shown in Table
2, ATPS, ADP, and UTP also transiently
increased
[Ca2+]i.
Significant differences in peak
[Ca2+]i
among ATP, ATPS, ADP, or UTP were not found. AMP and NECA did not
increase
[Ca2+]i.
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6 cm/s (Fig.
7A) and
remained constant at that elevated level during the whole observation
period. The addition of 10 µM ATP under Ca2+-free extracellular conditions
still caused a reduction of albumin permeability to 6.0 ± 0.7 × 106 cm/s and
evoked a transient rise of
[Ca2+]i
to a maximum of 500 nM (Fig. 7B).
Exposure of the endothelial cells to 300 nM thapsigargin in
Ca2+-free extracellular medium
discharged their endogenous Ca2+
stores (18, 22, 24) and was accompanied by a transitory small rise of
[Ca2+]i
and permeability that returned to basal level within 20 min. When
endothelial cells were exposed to 10 µM ATP after this maneuver was
completed, ATP no longer induced a rise in
[Ca2+]i.
Albumin permeability decreased nevertheless at the same velocity and to
the same extent as under control conditions in
Ca2+-free medium.
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ATP-induced effects on PKC, PLC, and permeability.
To analyze whether ATP causes activation of PKC, we isolated the
membrane fraction of ATP-stimulated endothelial cells and determined
the PKC activity in the native membrane-associated state. Exposure of
endothelial cells to 10 µM ATP for 10 min increased PKC activity in
the membrane fraction by 90% above the control level (Table
3). The increase in PKC activity in the
membrane fraction was virtually abolished when cells had been
pretreated for 20 min with 1 µM BIM, a panspecific inhibitor of PKC,
or 100 nM Gö-6976, a selective inhibitor of
Ca2+-dependent PKC isoenzymes
(Table 3). Exposure of endothelial cells to 1 µM BIM or 100 nM
Gö-6976 alone had no effect on basal PKC activity in the membrane
fraction.
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ATP-induced effects on cyclic nucleotides and permeability. We analyzed whether ATP stimulates cyclic nucleotide synthesis in endothelial cells and whether this synthesis is related to the ATP-induced reduction of macromolecule permeability.
Addition of 10 µM ATP to endothelial monolayers induced a rise in the cellular cGMP content within 5 min (Fig. 9B). Pretreatment of the endothelial cells for 10 min with 20 µM ODQ (29), a specific inhibitor of soluble guanylate cyclase, completely abolished the ATP-stimulated increase in cellular cGMP content. However, the ATP-induced reduction of macromolecule permeability was not changed in the presence of ODQ (Fig. 9A).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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The most prominent findings of the present study are that ATP induced a reduction of albumin permeability even though it provoked transient rises of [Ca2+]i, cGMP, cAMP, and translocation of PKC in porcine aortic endothelial monolayers. The ATP-induced rises of [Ca2+]i, cGMP, cAMP, and translocation of PKC could be prevented without abolishing the effect of ATP on permeability. The effect of ATP on permeability, however, was sensitive to inhibitors of PLC. These data show that ATP reduces macromolecule permeability via a PLC-mediated signaling pathway that is independent of concomitant effects on [Ca2+]i, cyclic nucleotides, or PKC.
Exposure of endothelial cells from the porcine aorta to ATP caused a
sustained reduction of albumin permeability. Similar effects were
observed in endothelial monolayers derived from the porcine pulmonary
artery, bovine aorta, and human umbilical vein. A detailed analysis was
carried out on endothelial cells from the porcine aorta. The effect of
ATP on barrier function was concentration dependent. ATPS, which is
much less hydrolyzable than ATP, reduced permeability in the same
manner as ATP, indicating that ATP, but not its degradation products,
caused the reduction of permeability. It has been reported (5, 21) that
ATP can stimulate endothelial cells via purinergic receptors, in
particular P2y and
P2u. The latter of these receptors
has a high affinity for UTP. In endothelial monolayers UTP also caused
a reduction of permeability in a concentration-dependent manner, but
this reduction was less potent than that induced by ATP. The fact that
the action of ATP can be mimicked by other nucleotides suggests that
ATP exerts its effect on permeability by acting on purinergic
receptors. The tested nucleotides were in the following rank order of
potency: ATP = ATPS > ADP = UTP. The order of potency is not
identical to that known for either P2y or
P2u. It may therefore correspond
to that of yet another one of the multitude of purinergic receptors
identified in cloning experiments.
To validate the conclusion that ATP and not a derivative is responsible for its effect on permeability, the actions of ATP, AMP, and the stable adenosine analog NECA were compared. We reported in a previous study (31) that NECA reduces endothelial albumin permeability via stimulation of endothelial adenosine receptors in the same model used in the present study. It has now been confirmed that NECA reduces endothelial permeability and that AMP has a comparable effect. Both effects could be fully antagonized by 8-PT, an adenosine-receptor antagonist. In contrast, 8-PT failed to antagonize the reduction of permeability obtained with ATP. These data therefore show independently that the effect of ATP on permeability is not due to the actions of adenosine.
In a further set of experiments, we tested the question of whether the reduction of permeability in the presence of ATP depends on the concomitant rise in [Ca2+]i. Two different experimental maneuvers were used. In the first maneuver, [Ca2+]i was kept at low intracellular levels during ATP stimulation by loading cells with the chelator BAPTA. In the second maneuver, endothelial cells were incubated in Ca2+-free medium and endogenous Ca2+ stores were preemptied by thapsigargin. It has been shown previously (24) that, with the latter protocol, the possibility of a rise in [Ca2+]i via extra- or intracellular causes is abolished. In the present study it was found that the loading of endothelial cells with BAPTA as well as extra- and intracellular Ca2+ deprivation completely precluded the ATP-evoked rise in [Ca2+]i, but these maneuvers did not affect the ATP-induced reduction of permeability. The experiments with the Ca2+ ionophore ionomycin show, from a different point of view, the dissociation between [Ca2+]i rise and reduction of permeability evoked by ATP. At the applied concentration, ionomycin causes a transient increase in [Ca2+]i that is comparable to the [Ca2+]i rise in the presence of ATP. The action of ionomycin circumvents the signal transduction activated by ATP that causes [Ca2+]i rise and a multitude of other effects (6). Experiments with ionomycin show that a sole rise in [Ca2+]i, without the other mechanisms also activated by ATP, causes a spontaneous increase in endothelial permeability. This is in accordance with many other observations (14-16, 18, 24). The contrasting effect of ATP must therefore be due to an intracellular mechanism activated in endothelial cells in response to ATP that overrides the Ca2+-activated increase in permeability.
It has been described previously (7, 27) that stimulation of endothelial cells with ATP causes activation of PLC. Here, we studied whether the activation of PLC is involved in the effects of ATP on permeability by using an inhibitor approach. The specific inhibitor of PLC, U-73122, was applied and compared with U-73343, an inactive analog of U-73122. The PLC inhibitor U-73122, but not its inactive analog, abolished the ATP-induced reduction of permeability. This indicates that the effect of ATP on permeability is mediated through activation of PLC. This conclusion is supported by the observation that ET-18-OCH3, a PLC inhibitor chemically distinct from U-73122, can also attenuate the ATP-induced reduction of permeability. Apart from its effect on permeability, U-73122 also abolished the increase in [Ca2+]i. This shows that the ATP-induced increase in [Ca2+]i, even though unrelated to permeability changes, is another PLC-dependent effect. Taken together, the experiments using the PLC inhibitors indicate that the permeability-reducing mechanism observed in the presence of ATP is activated on a level downstream of PLC but upstream of PLC-mediated [Ca2+]i rise.
PLC activation can lead to activation of PKC. A parameter of PKC
activation is translocation of PKC activity into cell membranes. In the
presence of ATP such an increase in membranous PKC activity was indeed
observed. This translocation was found to be abolished by pretreatment
of cells with the PKC inhibitor U-73122, indicating that it occurs
secondarily to PLC activation. PKC translocation was also inhibited in
the presence of the nonselective PKC inhibitor BIM or in the presence
of Gö-6976, an inhibitor of the
Ca2+-dependent isoforms of PKC.
This suggests that only
Ca2+-dependent isoforms are
translocated in response to stimulation with ATP. Endothelial cells are
known to express the
Ca2+-dependent PKC isoforms 
and (2).
In contrast to their effects on PKC translocation into the membrane fraction, the PKC inhibitors did not affect the ATP-induced rise in monolayer permeability. This indicates that the latter is independent of an activation of classic PKC isoforms that would all be inhibited by BIM. It leaves open the possibility that nonclassic isoforms of PKC are involved.
We found that the presence of ATP causes a transient rise in cGMP and cAMP in the cells. Processes that stimulate cGMP or cAMP synthesis may cause a reduction of macromolecule permeability of endothelial monolayers (17, 18). The changes in cyclic nucleotides, observed in the presence of ATP, could be blocked in the presence of specific inhibitors, ODQ for soluble guanylate cyclase and SQ-22536 for adenylate cyclase. The effects of the inhibitors indicate that the rises in cyclic nucleotides are due to activation of synthesis. We did not analyze this signaling of ATP stimulation toward cyclic nucleotide synthesis. Instead, we analyzed whether the changes in cAMP or cGMP contents affected the ATP-lowering effect on permeability. This was not the case. The ATP effect on permeability is thus independent of the changes in cyclic nucleotides.
In conclusion, ATP can stimulate both a rise in [Ca2+]i and a reduction of macromolecule permeability in the types of endothelial monolayers tested here. ATP seems to be the first mediator described that can exert such apparently contrasting effects. In general, rapid effects on endothelial permeability, as investigated here, seem to be due to two kinds of mechanisms: 1) a modulation of tension of the endothelial contractile machinery and 2) changes in cell-cell or cell-matrix adhesion. A transient rise of [Ca2+]i seems to increase endothelial permeability primarily by activation of the second type of mechanism (8). One may speculate that ATP overrides these [Ca2+]i-mediated effects on cell adhesion by the activation of specific Ca2+-independent signal transduction pathways. These have yet to be identified.
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ACKNOWLEDGEMENTS |
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This work was supported by the Deutsche Forschungsgemeinschaft Grant A3, A4 of SFB 547.
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FOOTNOTES |
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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. §1734 solely to indicate this fact.
Address for reprint requests and other correspondence: T. Noll, Physiologisches Institut, Justus-Liebig-Universität, Aulweg 129, D-35392 Giessen, Germany (E-mail: thomas.noll{at}physiologie.med.uni-giessen.de).
Received 16 November 1998; accepted in final form 1 February 1999.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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) and ATP (10 µM; 
) on albumin
permeability of aortic endothelial monolayers. 
, Control. Data are
means ± SD of n = 6 separate
experiments of independent cell preparations.
) on albumin permeability. 
,
Control (C). Data are means ± SD, after 20 min of incubation, of
n = 6 separate experiments of
independent cell preparations. At nucleotide concentrations
10
). Results
were compared with effects of ATP alone (10 µM; 
