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1 Department of Biomedical Engineering, Graduate School of Medicine, University of Tokyo, Tokyo 113-0033; and 2 Department of Physiology, Nagoya University School of Medicine, Nagoya 464-8601, Japan
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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ATP induces Ca2+ influx across the cell membrane and activates release from intracellular Ca2+ pools in vascular endothelial cells (ECs). Ca2+ signaling leads to the modification of a variety of EC functions, including the production of vasoactive substances such as nitric oxide and prostacyclin. However, the molecular mechanisms for ATP-induced Ca2+ influx in ECs have not been thoroughly clarified. Here we demonstrate evidence that a P2X4 receptor for an ATP-gated cation channel is predominantly expressed in human ECs and is involved in the ATP-induced Ca2+ influx. Northern blot analysis distinctly showed the expression of P2X4 mRNA in human ECs cultured from the umbilical vein, aorta, pulmonary artery, and skin microvessels. Competitive PCR revealed that P2X4 mRNA expression was much higher in ECs than was the expression of other subtypes, including P2X1, P2X3, P2X5, and P2X7. Treatment of ECs with antisense oligonucleotides designed to target the P2X4 receptor decreased the P2X4 mRNA and protein levels to ~25% of control levels and markedly prevented the ATP-induced Ca2+ influx.
purinoceptor; antisense oligo; ion channel; adenine nucleotide
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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CA2+ signaling plays an important role in agonist- or hemodynamic stress-mediated regulation of endothelial cell (EC) functions. An increase in intracellular Ca2+ concentrations ([Ca2+]i) has been observed in ECs stimulated with agonists such as ATP, histamine, bradykinin, and thrombin (8, 10) and also in ECs exposed to hemodynamic stresses such as shear stress and cyclic stretch (1, 18, 25). When [Ca2+]i increases, Ca2+-binding proteins (such as the specific receptor calmodulin) bind to Ca2+, and the Ca2+-protein complexes then interact with other proteins in the cell to alter their functions. This results in changes in EC functions such as increased nitric oxide and prostacyclin production, which cause vasodilatation. Recent studies (2, 4) indicate that differences in the amplitude and duration of a [Ca2+]i increase contribute to the differential activation of various transcription factors.
The pattern of an increase in [Ca2+]i induced by ATP usually consists of a peak and a sustained phase (8). The peak is caused by the Ca2+ release from intracellular Ca2+ stores, and the sustained phase is due to the influx of extracellular Ca2+ across the cell membrane. The Ca2+ release is known to be mediated by P2 purinoceptors such as P2Y1 and P2Y2 (20). Binding of extracellular ATP to these receptors activates phospholipase C via GTP-binding protein and generates D-myo-inositol 1,4,5-trisphosphate [Ins(1,4,5)P3], which triggers Ca2+ release from intracellular Ca2+ stores. The molecular mechanism for ATP-induced Ca2+ influx remains unclear, but the involvement of D-myo-inositol 1,3,4,5-tetrakisphosphate [Ins(1,3,4,5)P4]-sensitive cation channels (17) or Ca2+-release-activated channels (11) has been suggested.
The recently discovered family of ligand-gated channels activated by extracellular ATP, the P2X receptors, is widely distributed in visceral and vascular smooth muscle cell types, as well as in numerous neuronal and glial cell types (3, 5). Seven different genes encoding P2X receptors have been identified in rat (rP2X1, rP2X2, rP2X3, rP2X4, rP2X5, rP2X6, and rP2X7) and five human homologue receptors (hP2X1, hP2X3, hP2X4, hP2X5, and hP2X7) have been characterized. Each P2X receptor subunit appears to have a common three-dimensional structure: two hydrophobic putative transmembrane domains with an intervening hydrophilic loop of almost 300 amino acids lying on the extracellular surface and intracellular NH2 and COOH terminals. The P2X receptors, however, have never been reported to be expressed in vascular ECs. In this study, we investigated whether human vascular ECs express P2X purinoceptors, and if so, which subtype is predominantly expressed. Furthermore, to examine the role of P2X purinoceptors in the mechanism for the ATP-induced Ca2+ response, we inhibited P2X gene expression with antisense oligonucleotides.
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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All animals were handled in accordance with the guidelines approved by the Animal Research Committee, University of Tokyo, which follow the guidelines outlined by the American Physiological Society.
Cell culture. Primary cultures of human umbilical vein ECs (HUVECs) were obtained from human umbilical cord veins by collagenase treatment, and ECs from aorta (HAECs), pulmonary artery (HPAECs), and microvessel (HMVECs) were purchased from Clontech. All ECs were cultured on a 1% gelatin-coated flask in medium-199 (ICN Biomedicals) containing 15% fetal bovine serum (GIBCO-BRL), 2 mM L-glutamine (GIBCO-BRL), 50 U/ml penicillin, 50 µg/ml streptomycin (ICN Biomedicals), 50 µg/ml heparin (Sigma), and 30 µg/ml EC growth factor (Becton-Dickinson) in an atmosphere of 5% CO2 at 37°C. Cells were routinely passaged by trypsinization (ICN Biomedicals); those used for the present experiments were obtained during the fourth and tenth passages.
Cloning and sequencing of the P2X4 receptor.
Human lung total RNA (Clontech) was amplified by RT-PCR using sense and
antisense primers for the P2X4 receptor (Table
1) (6). The P2X4
cDNA fragment was radiolabeled with [
-32P]dCTP using a
random primer labeling kit (Takara). An HUVEC cDNA library (Clontech)
was screened by lifting 1.2 × 106 phages onto a
Hybond-N nylon membrane (Amersham). After 12 h of prehybridization
in 5× SSC (1× SSC is 750 mM sodium chloride and 75 mM sodium citrate,
pH 7.0) (24), 5× Denhardt solution, 0.5% SDS, 10%
dextran sulfate, and 0.25 mg/ml salmon testis DNA at 65°C,
hybridization was carried out in the same solution with a radiolabeled
P2X4 probe for 20 h at 65°C. The positive clones were identified by autoradiography on X-ray film. The DNA from the
positive clones was isolated, digested with EcoR I, and
subcloned into a pBluescript II vector (Stratagene). The complete
nucleotide sequence was determined using DNA sequencer 373S-36 (Applied
Biosystems). The sequence is the same as was previously reported from
other tissues, and the GenBank accession number is AF000234.
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Northern blot analysis. mRNA was obtained from HUVECs, HAECs, HPAECs, and HMVECs using the MACS mRNA Isolation Kit (Miltenyi Biotec). Briefly, cells were lysed with a high-salt buffer containing 1% SDS. Colloidal super-paramagnetic MicroBeads conjugated to oligo(dT) were added to the lysed cells, and the lysate was passed through the magnetic field of the MACS separator column. mRNA that was hybridized to the oligo(dT) MicroBeads remained in the column. After the column was washed to remove protein, DNA, and rRNA, the pure mRNA was eluted using elution buffer.
We fractionated 2 µg of mRNA on a 1% agarose-6% formaldehyde gel with 0.02 M MOPS buffer (Sigma), 5 mM sodium acetate, and 1 mM EDTA. The fractions were capillary transferred to noncharged nylon membranes and were ultraviolet (UV) cross-linked. After 30 min of prehybridization at 68°C in ExpressHyb hybridization solution (Clontech), the membrane was hybridized with an [-32P]dCTP scrambled primed P2X4 DNA
probe, which was obtained from the cloning previously described. The
blot was washed with 2× SSC and 0.05% SDS and visualized with a GS363
Molecular Imager System (Bio-Rad).
RT-PCR analysis.
Competitive PCR was used to compare mRNA levels of P2X subtypes.
Heterologous competitors for the P2X1, P2X3,
P2X4, P2X5, P2X7, P2Y1,
and P2Y2 genes were generated using the Competitive DNA
Construction Kit (Takara). Both sense and antisense primers were
synthesized. The sense primers consisted of the gene-specific sense
sequence (Table 1) with an additional SP6 promoter sequence at the 5'
end and a composite sense primer at the 3' end used only for competitor
construction. The antisense primers were made up of each gene-specific
antisense sequence, linked at the 3' end to a composite antisense
primer. With the use of these primers, DNA competitor fragments were
obtained by PCR amplification (30 cycles of 30 s at 94°C,
30 s at 60°C, and 45 s at 70°C). The DNA fragments were
then transcribed into RNA fragments using SP6 RNA polymerase
(Competitive RNA Transcription Kit, Takara). The RNA competitor
fragments were extracted with phenol, chloroform, and isoamyl alcohol
and precipitated with ethanol. The RNA concentration was determined
spectrophotometrically and diluted to 800 amol/µl. Initially,
competitive PCR was performed by adding 2 µl of the mRNA samples
obtained from HUVECs or HAECs to 2 µl of different 10-fold dilutions
of the RNA competitor fragments ranging from 0.00008 to 800 amol/µl
(13). The mixture was kept at 37°C for 1 h and
heated to 99°C for 5 min in the presence of Moloney murine leukemia
virus RT (GIBCO-BRL), oligo(dT)12-18, RNase inhibitor, each dNTP mixture, and dithiothreitol in a first-strand buffer. After
reverse transcription, the PCR reactions were carried out using each
target gene-specific primer (Table 1) in a solution containing
ExTaq DNA polymerase (Takara) and
[-32P]dCTP. Each temperature cycle consisted
of 95°C for 30 s, 60°C for 30 s, and 72°C for 1 min.
The sequences of the PCR products showed that each mRNA was correctly
amplified by those primers. A second series of competitive PCR assays
was then carried out with consecutive 1:2 dilutions of competitors
mixed with a constant amount of each target mRNA. The PCR products were
separated by electrophoresis in a 5% polyacrylamide gel. The
radioactivity of both target mRNA bands and competitor bands (known
concentrations) was measured with a GS363 Molecular Imager System. The
logarithm of the ratio of target bands to competitor bands was plotted
as a function of the logarithm of the known amounts of competitor. The
concentration of target mRNA molecules present in ECs corresponds to
that of competitor at the competition equivalence point
[log(target/competitor) = 0]. The 
-actin gene, which is a
housekeeping gene, was used as a control for variation in RNA quality
and quantity.
Generation of the P2X4 antibody. An antiserum against human P2X4 receptor protein was generated in rabbits injected with a synthetic peptide (NH2-RLYYREKKYKYVEDYC-COOH) comprising amino acid residues 364-378 of the sequences for the intracellular COOH-terminal domains of the cloned human P2X4 receptor. Peptide was covalently linked to keyhole limpet hemocyanin, and rabbits were immunized by injection with the conjugated peptide every 2 wk for 8 wk. The anti-P2X4 receptor antiserum was then affinity purified using a synthetic peptide (P2X4 residues 364-378) immobilized on Sepharose 4B (Asahi Techno Glass).
Western blot analysis.
HUVECs were washed with cold PBS and solubilized in 500 µl
radioimmunoprecipitation assay (RIPA) buffer (1% Nonidet P-40, 20 mM
Tris · HCl, 0.15 M NaCl, 0.5% sodium deoxycholate, 2 mM EDTA, 2 mM EGTA, 0.1% SDS, 0.2 mM Na2MoO4, 10 mM NaF,
1 mM Na3VO4, 1 mM phenylmethylsulfonyl
fluoride, 5 µg/ml leupeptin, 5 µg/ml antipain, 5 µg/ml pepstatin
A, and 0.2 U/ml aprotinin; pH 7.4). Lysates were centrifuged at 26,000 g for 30 min. The supernatants were immunoprecipitated using
the anti-P2X4 receptor antiserum, which was prebound to
protein A-Sepharose beads (Millipore, Bedford, MA). After four washes
with RIPA buffer, immunoprecipitated proteins were solubilized in SDS
sample buffer (0.2 M Tris · HCl, 18% glycerol, 4% SDS, 0.01%
bromphenol blue, and 10% -mercaptoethanol; pH 8.8) for SDS-PAGE.
Gels were transferred to Immobilon polyvinylidene difluoride membranes
(Millipore). Membranes were blocked in Tris-buffered saline with 5%
skim milk and 0.1% Tween 20 and then incubated for 1 h with the
anti-P2X4 antiserum (3 µg/ml). Membranes were washed in
PBS and incubated with anti-rabbit IgG horseradish
peroxidase-conjugated antibody. The blots were developed using an
enhanced chemiluminescence kit (Amersham) and analyzed by the GS363
Molecular Imager (Bio-Rad).
Antisense oligonucleotides. Antisense oligonucleotides (AS-oligos) targeted to the P2X4 receptor and scrambled control oligos (S-oligos) were designed and synthesized by Biognostik (Göttingen, Germany). Sequences of phosphorothioated AS-oligos and S-oligos were 5'-CCTGAAATTGTAGCC-3' and 5'-TAATCGCTTCAGACG-3', respectively, and were FITC labeled at the 5' end. AS-oligos or S-oligos were transfected into cells using LipofectAMINE PLUS (GIBCO-BRL). Cellular uptake of AS-oligos was checked by the observation of FITC using a fluorescence microscope.
[Ca2+]i determination. ECs, which were cultured on a 40-mm-diameter round coverslip coated with 1% gelatin, were loaded with indo 1-acetoxymethylester (Dojindo). The coverslip was placed in the FCS2, a parallel plate type of flow chamber (Bioptechs, Butler, PA), on the stage of an inverted microscope (Diaphot 300, Nikon). Agonists in Hanks' balanced salt solution were perfused through the chamber (using a peristaltic pump) at a flow rate of 3 ml/min to stimulate cells at 37°C.
Agonist-induced changes in [Ca2+]i were monitored with a confocal laser scanning system (MRC-1000 UV, Bio-Rad) equipped with an UV argon ion laser, as has been previously described (12). Briefly, 351-nm wavelength light from the laser excited cells through a ×40 objective. The emitted light was separated into 405- and 480-nm wavelengths by a beam splitter and was counted using photomultipliers. The time course of the F405/F480 fluorescence ratio in cells of interest was monitored using the accessory time course software of the Bio-Rad 1000 UV system.Statistical analysis. Differences in [Ca2+]i between the control and antisense-treated cells were evaluated by ANOVA, followed by Bonferroni modification of the t-test by using SPSS. Significance was assumed at P < 0.05.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Vascular ECs express the P2X4 receptor.
Northern blot analysis using the P2X4 cDNA probe
demonstrated that P2X4 mRNA was expressed in HUVECs, HAECs,
HPAECs, and HMVECs (Fig. 1). However,
another P2X subtype P2X1 was not expressed in any of these
EC lines.
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AS-oligo knockout of P2X4 receptor expression in ECs.
To assess the physiological role of P2X4 receptors in ECs,
we used AS-oligos to specifically knock out P2X4 receptor
function. When HUVECs were treated with the AS-oligos, P2X4
receptor mRNA and protein levels decreased to ~25% of control
levels, although neither changed after S-oligo treatment (Fig.
3). The AS-oligos had no effect on the
levels of P2X1, P2X3, P2X5,
P2X7, P2Y1, or P2Y2 mRNA expression
(Fig. 4), indicating that the AS-oligos
specifically knock out the expression of P2X4 receptors.
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P2X4 receptors mediate ATP-induced Ca2+
influx in ECs.
When HUVECs were stimulated with ATP (4 µM), they showed an initial
peak and subsequent sustained phase in
[Ca2+]i (Fig.
5A). HUVECs treated with
S-oligos showed almost the same Ca2+ response pattern as
observed in the control cells (Fig. 5B). On the other hand,
HUVECs treated with AS-oligos showed an initial peak but no subsequent
sustained phase in [Ca2+]i (Fig.
5C). This Ca2+ response pattern was quite
similar to that seen in the absence of extracellular Ca2+
(Fig. 5, D-F), indicating that Ca2+
influx was inhibited in AS-oligo-treated cells. This was confirmed by a
quantitative analysis of the ATP-induced Ca2+ responses
(Fig. 6). The same phenomenon was also
observed in HAECs and HPAECs (data not shown). These findings indicate
that the P2X4 receptor mediates ATP-induced
Ca2+ influx in human ECs.
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P2X4 receptors are not involved in histamine-induced
Ca2+ influx.
Histamine induced an initial peak and subsequent sustained phase in
[Ca2+]i, which is quite similar to that seen
in ATP stimulation (Fig. 8). Treatment of
HUVECs with the P2X4 receptor AS-oligos, however, did not
affect the histamine-induced Ca2+ response. This suggests
that Ca2+-permeable cation channels other than
P2X4 receptors are involved in the histamine-induced
Ca2+ influx.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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The present study is the first to demonstrate that cultured human vascular ECs express P2X4 receptors, which are ATP-gated ion channels that mediate Ca2+ influx induced by ATP. P2X receptors are widely distributed in various tissues of mammals, including smooth muscle of the urinary bladder and arteries, kidney, pancreas, lung, cardiac myocytes, sensory and sympathetic ganglia, and brain and spinal cord. Five genes encoding the human P2X receptor subtypes (P2X1, P2X3, P2X4, P2X5, and P2X7) have been cloned (6, 7, 14, 16, 23, 27). Each subtype seems to be preferentially expressed in different tissues. For instance, the rP2X1 receptor is predominantly localized to smooth muscles, but the rP2X2 receptor, which is not expressed in smooth muscles, is found predominantly in neurons (5). In this study, Northern blot analysis showed expression of P2X4 mRNA in cultured human ECs from umbilical vein, aortic, pulmonary artery, and microvessel but failed to detect P2X1 transcripts. Competitive PCR using sense and antisense primers for these P2X receptor subtypes revealed that the level of P2X4 mRNA was significantly higher than that of any of the other subtypes in cultured human ECs. Western blot analysis and fluorescence immunostaining (data not shown) using an anti-P2X4 polyclonal antibody showed that HUVECs also express P2X4 at protein levels. These results suggest that HUVECs predominantly express P2X4 receptors.
Because there are no specific inhibitors available, we used AS-oligos to selectively interfere with P2X4 to assess its physiological role in ECs. Treatment of ECs with the AS-oligos markedly decreased P2X4 mRNA levels but did not change the mRNA levels of other subtypes, including P2X1, P2X3, P2X5, P2X7, P2Y1, and P2Y2. Western blots using an anti-P2X4 polyclonal antibody confirmed that protein levels of the P2X4 receptor were also decreased in the AS-oligo-treated ECs. Treatment of ECs with S-oligos had no effect on the P2X4 mRNA or protein levels. Attenuation of P2X4 activity by AS-oligos was reversed by incubating AS-oligo-treated cells in normal media for 1 wk, indicating that the effect of AS-oligos was temporary (data not shown). The AS-oligos were not toxic to ECs and did not cause any change in cell morphology, as assessed by trypan blue dye exclusion test and phase-contrast microscopy. Taken together, AS-oligos may be used to effectively and selectively disrupt P2X4 receptor function in ECs.
When P2X4 expression was inhibited by the AS-oligos in HUVECs, the ATP-induced increase in [Ca2+]i, especially the sustained phase, was markedly suppressed. This phenomenon was also observed in HAECs and HPAECs. These results indicate that P2X4 receptors contribute to ATP-induced Ca2+ influx in ECs. The inhibitory effect of AS-oligos on the ATP-induced Ca2+ influx varied depending on the [ATP] used. At <4 µM ATP, the Ca2+ influx was almost abolished, and at >4 µM ATP, it was partially inhibited. Because AS-oligos do not completely knock out P2X4 expression in ECs (as shown in Fig. 3), high doses of ATP may activate the remaining P2X4 receptors to induce Ca2+ influx. High doses of ATP may also open other P2X subtypes, such as P2X7, or activate unknown Ca2+-permeable channels other than P2X receptors. The Ca2+ influx seen at high [ATP] may also be due to store-operated Ca2+ influx (capacitative Ca2+ entry) triggered by P2Y-mediated Ca2+ release from Ca2+ stores (21). Recently the transient receptor potential protein has been found to form store-operated cation channels in human ECs (9, 28). Furthermore, high doses of ATP may inhibit Ca2+ removal from the cytoplasm or prolong Ca2+ release from the intracellular Ca2+ store. Histamine induces a [Ca2+]i peak and a sustained phase in ECs that are similar to those seen with ATP stimulation. Because the P2X4 AS-oligos had no effect on the histamine-induced Ca2+ response, cation channels other than the P2X4 receptor seem to be involved in the histamine-induced Ca2+ influx. These results indicate that channels responsible for agonist-activated Ca2+ influx may vary with different agonists. Further studies are needed to determine how P2Y-mediated Ca2+ release and influx are related to P2X4 receptor-mediated Ca2+ influx in ECs.
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ACKNOWLEDGEMENTS |
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We sincerely thank Dr. Y. Takada, Asahi Chemical Industry, for advice.
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FOOTNOTES |
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This work was partly supported by Grants-in-Aid for Scientific Research and for Scientific Research on Priority Areas from the Japanese Ministry of Education, Science, and Culture, a research grant for cardiovascular diseases from the Japanese Ministry of Health and Welfare, Special Coordination Funds for Promoting Science and Technology, and research funds from the Program for Promotion of Fundamental Studies in Health Sciences of the Organization for Drug ADR Relief, R&D Promotion, and Product Review of Japan.
Address for reprint requests and other correspondence: J. Ando, Dept. of Biomedical Engineering, Graduate School of Medicine, Univ. of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033 Japan (E-mail: joji{at}m.u-tokyo.ac.jp).
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.
Received 22 October 1999; accepted in final form 11 January 2000.
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RESULTS
DISCUSSION
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10 µM).
