From the Laboratory of Pharmacology, Brussels University School of Medicine, Brussels, Belgium
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ABSTRACT |
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INTRODUCTION |
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Cytosolic Ca2+ has also been implicated as a proapoptotic agent involved in triggering apoptosis and regulating death-specific enzymes (2). Apoptosis, also known as programmed cell death, plays a major role in the normal development of most organs (3). However, too much or too little apoptosis is also implicated in a large number of clinical disorders, including ischemia, cancers, type 1 diabetes, neurodegenerative disorders such as Alzheimers disease, and viral infections, e.g., HIV-1 (4). The family of cysteine proteases, known as caspases, are critical mediators of apoptosis (5) that can be triggered by three distinct pathways: oligomerization of death receptors located on the plasma membrane, mitochondrial damage, and the recently discovered endoplasmic reticulum (ER) pathway (6,7). In the latter triggering mechanism, "ER stress," including disruption of ER Ca2+ homeostasis or accumulation of excess protein in the ER, causes the activation of caspase-12 (8) that triggers the process of apoptosis (7). Therefore, the development of strategies to control intracellular Ca2+ homeostasis may represent a potential approach to prevent or enhance programmed cell death. This could be accomplished by overexpressing the Na/Ca exchanger, an ubiquitous mechanism for Ca2+ extrusion from excitable and nonexcitable cells (9).
In the present study, we examined the effect of Na/Ca exchanger overexpression on Ca2+-induced apoptosis in insulin-producing cells. Indeed, Ca2+ plays a major role in the process of insulin release from the pancreatic ß-cell (10), and in type 1 diabetes (insulin dependent), the autoimmune destruction of pancreatic ß-cells appears to be mediated by apoptosis (11), a phenomenon that could involve Ca2+. Thus, serum from newly diagnosed type 1 diabetic subjects was shown to activate Ca2+ inflow in mouse ß-cells through voltage-sensitive Ca2+-channels and to promote ß-cell destruction by apoptosis (12). Likewise, chronic cytokine treatment (interleukin-1ß plus interferon-) induces a low voltageactivated Ca2+ current in mouse islet cells, a phenomenon associated with a sustained increase in basal intracellular calcium concentration ([Ca2+]i) and apoptotic cell death (13). Glucose itself, the main physiological stimulus of insulin release, when used at a high concentration (17 or 27 mmol/l), was observed to trigger apoptosis in both mouse and rat ß-cells, a process that again was Ca2+-dependent (14).
The pancreatic ß-cell is equipped with two systems allowing Ca2+ extrusion, the plasma membrane Ca2+-ATPase (PMCA) and the Na/Ca exchanger (15,16). The latter system couples the electrogenic transport of 3 Na+ ions for 1 Ca2+ ion (9). In rat ß-cells, like in cardiac myocytes, Na/Ca exchange is the major mechanism for Ca2+ extrusion (17,18) and participates in the control of [Ca2+]i and of insulin release (18,19).
The Na/Ca exchanger (NCX) was cloned 10 years ago, and three mammalian isoforms have been identified: NCX1, -2, and -3. Several splice variants of NCX1 and -3 have been described, each exhibiting a specific tissue distribution (reviewed in 20). Rat pancreatic islet cells, purified ß-cells, and the insulinoma cell line (RINm5F cells) express two NCX1 splice variants (NCX1.3 and -1.7).
In the current study, apoptosis rates were determined in an insulin-secreting cell line (BRIN-BD11) overexpressing the human NCX1.7 exchanger isoform (21). BRIN-BD11 cells, produced by electrofusion of normal rat pancreatic ß-cells and RINm5F cells (22), were chosen instead of RINm5F cells because they show a fully functional glucose responsiveness and do not suffer from the inherent defect recorded with parental RINm5F cells (22). Our data reveal that overexpression of the exchanger depletes ER Ca2+ stores, a phenomenon that leads to ER stress, activation of caspase-12, and increase in Ca2+-mediated apoptosis. Overexpression of the exchanger also reduced cell proliferation and sensitized the cells to nonCa2+-dependent apoptotic signals.
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RESEARCH DESIGN AND METHODS |
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Except otherwise stated, all experiments were carried out in complete RPMI medium in a humidified atmosphere of 5% CO2/95% air at 37°C. Likewise, all viability/cytotoxic/apoptotic assays were carried out over 48 h, except nuclear chromatin staining and caspase-12 activation assay, which were carried out over 24 h.
Cell viability/cytotoxicity assay.
Control cells and cells overexpressing the Na/Ca exchanger were seeded at 1.5 x 105 cells/ml, cultured overnight in flat-bottom 96-well plates, and treated with a variety of agents known to induce apoptosis and/or to affect [Ca2+] i. Cell viability/cytotoxicity was determined by the 3-(4,5-dimethylthiazol-2yl)-2,5-diphenyl tetrazolium bromide (MTT) assay as previously described (23). This assay is based on the ability of viable cells, but not death cells, to reduce MTT, with the reaction generating a dark blue insoluble formazan product. Briefly, after exposure of the cells to the different agents for 48 h, 10 µl MTT in PBS (5 mg/ml) were added to 100 µl medium in each well and further incubated for 4 h. A total of 100 µl of 40 mmol/l HCl/isopropanol was then added to stop MTT reduction and to dissolve the dye. After a 10-min incubation at 37°C, colorimetric measures were made at 540 nm with an ELISA (enzyme-linked immunosorbent assay) plate reader (Labsystems Oy, Helsinki, Finland). Results are expressed as percentage of absorbances relative to controls (defined as 100%) after subtraction of noncell-derived background.
Nuclear chromatin staining.
Cells were cultured overnight on circular cover glasses at 2.5 x 105 cells/ml in complete RPMI medium and treated with the previously mentioned agents for 24 h. The incubation time was 24 instead of 48 h because apoptotic cells usually detach from the culture plates and hence escape detection. After washing with PBS, cells were incubated in PBS containing Hoechst 33342 (20 µg/ml) for 10 min at 37°C. The dye was then removed, and apoptotic cells were identified by the presence of condensed nuclei, which were stained blue and visualized using a fluorescent microscope (UV excitation at 340380 nm) (14).
Quantification of DNA fragmentation.
Cells (2.5 x 105 cells/ml) were washed with Hanks balanced salt solution, detached using nonenzymatic cell dissociation buffer, and collected by centrifugation. Fragmented DNA was isolated and quantified as previously described (24), with some modifications. A total of 300 µl lysis buffer (0.5% Triton X-100, 20 mmol/l EDTA, and 5 mmol/l Tris-HCl; pH 7.4) was added to the cells. After 20 min incubation at 4°C, cells were centrifuged at 15,000g for 30 min. Pellets were resuspended in 300 µl lysis buffer containing 100 µg Proteinase K. Sixty micrograms of Proteinase K was also added to the supernatants. Samples were incubated overnight at 37°C with gentle shaking, and DNA was extracted with phenol-chloroform. Each DNA fraction was incubated in TNE buffer (10 mmol/l Tris-HCl, 200 mmol/l NaCl, and 1 mmol/l EDTA; pH 7.4) in the presence of Hoechst 33258 at 0.5 µg/ml. Fluorescence of fragmented (supernatant) and nonfragmented DNA (pellets), respectively, was measured with a spectrofluorometer (excitation at 356 nm and emission at 492 nm). Results were expressed as percent of fragmented DNA.
Gel electrophoresis of low molecular weight DNA.
DNA extraction was performed as described above. After ethanol precipitation, fragmented DNA was incubated in 30 µl TER buffer (10 mmol/l Tris-HCl, 1 mmol/l EDTA, and 2 µg/ml RNAse A; pH 8) for 1 h at 37°C with gentle shaking. Samples were run on 1.2% agarose gels. DNA was visualized by ethidium bromide staining (24).
Cytosolic Ca2+ concentration measurements.
Cells previously plated on round glass coverslips were incubated with fura-2 acetoxymethyl ester (final concentration 2 µmol/l) during 60 min at 37°C in Krebs-Ringer bicarbonatebuffered solution supplemented with glucose (2.8 mmol/l). The coverslips were then transferred to a tissue chamber mounted on an inverted fluorescence microscope (Diaphot TDM; Nikon, Tokyo) for epifluorescence. Fura-2 fluorescence of single cells was measured by dual-excitation fluorimetry using a camera-based image analysis system (Magical; Applied Imaging, Sunderland, U.K.). The excitation and emission wavelengths were set at 340/380 and 510 nm, respectively, and a pair of ratioable images (at the excitations of 340 and 380 nm, 30-ms interval) were taken every 2.5 s. [Ca2+]i was calculated from the ratios of the 340- and 380-nm signals as previously described (18).
Measurements of the Ca2+ concentration in the ER.
Furaptra loading, permeabilization, and measurements of intracellular Ca2+ stores were performed as previously described (25), with some modifications. Briefly, cells were loaded with furaptra acetoxymethyl ester (4 µmol/l) and 0.05% (wt/vol) Pluronic F-127 in Krebs-Ringer bicarbonatebuffered solution supplemented with glucose (2.8 mmol/l) for 60 min at 37°C. After rinsing, round glass coverslips with the attached cells were then transferred to a tissue chamber mounted on an inverted fluorescence microscope. Permeabilization of the plasma membrane was carried out with 4 µ mol/l digitonin in intracellular medium containing 140 mmol/l KCl, 10 mmol/l Na2ATP, and 10 mmol/l HEPES, pH 7.0, adjusted with KOH. Free Ca2+ was buffered at 200 nmol/l with 2 mmol/l EGTA and the appropriate amount of Ca2+ using the Max Chelator program (Stanford University). Furaptra fluorescence of single loaded cells was measured by use of dual-excitation microfluorimetry with a SPEX photometric system (Optilas, Alphen aan den Rijn, Holland). The excitation wavelengths (340 and 380 nm) were alternated at the frequency of 1 Hz. The emission wavelength was set at 510 nm. After the sudden drop of fluorescence, the detergent was removed and intracellular buffer was added. Thapsigargin (1 µ mol/l) was used to estimate the content of free Ca2+ in the ER.
Western blot analysis.
Approximately 3 x 106 cells were collected and lysed in lysis buffer (NP40 1%, TRIS 10 mmol/l, NaCl 200 mmol/l, EDTA 5 mmol/l, glycerol 10%, and protease inhibitors; pH = 7). Lysates containing 25 µg protein were run on 12% acrylamide gels, transferred onto nitrocellulose, and analyzed (21) using a 1/1,000 dilution of a polyclonal antibody raised against caspase-12 (kindly supplied by P. Vandenabeele, Department of Molecular Biology, University of Ghent, Ghent, Belgium). Because caspase-12 activation is an early process, cells were exposed to apoptotic agents for 24 h.
Caspase activity detection using fluorescence microscopy.
Caspase activity was measured using the Caspatag fluorescein Caspase (VAD) activity kit (Intergen, Oxford, U.K.) and fluorescence microscopy. The cells were plated on sterile glass coverslips for 24 h and further incubated for 48 h in the absence or presence of 1 µ mol/l thapsigargin. Cells were then incubated for 1 h at 37°C under 5% CO2 with the fluorescent caspase inhibitor FAM-VAD-FMK. The medium was then removed and cells washed twice with wash buffer. The coverslips were mounted on a slide using a drop of wash buffer and observed under a fluorescence microscope (Olympus AX70 System Microscope; Omnilabo, Aartselaar, Belgium) to view green fluorescence of caspase-positive cells (excitation at 490 nm and emission at 520 nm.).
Cell proliferation assay.
Cells were seeded at 1.5 x 105 cells/ml and cultured for 24 h in flat-bottom 96-well plates in the absence of FCS. Cells were then incubated with 0, 3, 6, and 10% of FCS during 48 h to measure serum-induced proliferation using the MTT assay as described above and by cell counting using trypan blue and a Bü rcher cell. All data are expressed as means ± SE. Statistical significance of differences between data were assessed by using ANOVA and Tukeys post test.
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RESULTS |
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The agents used to increase [Ca2+] i comprised glucose and the hypoglycemic sulfonylureas tolbutamide and glibenclamide, the sarco(endo)plasmic reticulum Ca2+-ATPase (SERCA) inhibitors thapsigargin and cyclopiazonic acid (CPA), and the ionophore ionomycin. Glucose and the hypoglycemic sulfonylureas increase [Ca2+] i by closing ATP-dependent K+ channels, which depolarize the plasma membrane, open voltage-sensitive Ca2+ channels, and hence increase Ca2+ inflow (26). SERCA inhibitors block the ER Ca2+-ATPases and increase [Ca2+]i by releasing Ca2+ from the ER (27). Ionomycin acts as a Ca2+ ionophore, namely by permeabilizing the plasma membrane and the intracellular membranes to Ca2+, and hence increases both Ca2+ inflow from the outside and the release of the ion from intracellular stores.
The MTT assay was used to measure cell viability. Figure 1A illustrates the effect of various agents increasing [Ca2+] i on cell viability. In control cells, SERCA inhibitors (thapsigargin and CPA) decreased cell viability (P < 0.001), whereas the hypoglycemic sulfonylureas glibenclamide and tolbutamide did not. The ionophore ionomycin decreased cell viability but only at the highest concentration used (6 µmol/l, P < 0.001). In cells overexpressing the Na/Ca exchanger, the effect of SERCA inhibitors was increased (P < 0.001), whereas that of ionomycin (3 and 6 µmol/l) and the hypoglycemic inhibitors was not. Similar data were obtained using another independent clone overexpressing NCX1.7 (data not shown). In cells transfected with the expression vector lacking the NCX1.7 construct, the effect of thapsigargin or CPA on cell viability was not different from that observed in nontransfected cells (P > 0.05) (Fig. 1A hatched columns). Figure 1B illustrates the time course of the effect of thapsigargin and CPA on cell viability. In overexpressing cells, there was a shift to the left in the time dependence of the two inhibitors inducing apoptosis, confirming that overexpression sensitizes the cells to apoptotic cell death. For instance, with thapsigargin, a significant decrease in cell viability was observed after 12 and 24 h in overexpressing and control cells, respectively (P < 0.001). With CPA, a significant decrease in cell viability was observed after 6 and 24 h in overexpressing and control cells, respectively (P < 0.001).
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One of the hallmarks of apoptosis is nuclear DNA fragmentation into oligonucleosomal fragments, which can be visualized as a DNA ladder by agarose gel electrophoresis. In contrast, DNA electrophoresis of necrotic cells yields a "smear" pattern due to random DNA degradation. Using this method, we observed that thapsigargin and CPA cause cell death by apoptosis rather than by necrosis in both control and Na/Ca exchangeroverexpressing cells (Fig. 3A). Fragmented DNA was not visible in untreated cells and cells treated with sulfonylureas (100 µmol/l tolbutamide and 10 µmol/l glibenclamide) or ionomycin (3 µmol/l). At 6 µmol/l, ionomycin induced DNA fragmentation, but only in Na/Ca exchanger overexpressing cells.
To examine the mechanism by which Na/Ca exchanger overexpression favors apoptosis, the effect of SERCA inhibitors and ionomycin on [Ca2+]i was evaluated (Fig. 4). In control cells, thapsigargin and CPA induced a major but transient increase in [Ca2+]i, a phenomenon that was reduced by 60 and 40%, respectively, in Na/Ca exchangeroverexpressing cells (P < 0.0001). On the contrary, in cells transfected with the expression vector lacking the NCX1.7 construct, the effect of thapsigargin and CPA on [Ca2+]i was slightly larger, although not significantly so, than that observed in control nontransfected cells (P > 0.1 and 0.075, respectively) (Fig. 4). In control cells, ionomycin induced an even more marked increase in [Ca2+]i; the increase was also more sustained than that induced by SERCA inhibitors. In Na/Ca exchangeroverexpressing cells, ionomycin also increased [Ca2+]i, but the increase was more sluggish. However, at steady state, the rise in [Ca2+]i was of the same magnitude in control and overexpressing cells (Fig. 4, lower left panel). Tolbutamide also increased [Ca2+] i; the pattern of rise was similar to that of ionomycin, except that it was of a lower magnitude. Thus, in overexpressing cells, the increase was more progressive but of similar magnitude at the steady state compared with control cells (P > 0.05) (Fig. 4D). Taken as a whole, these data show that overexpression of the Na/Ca exchanger reduces the rise in [Ca2+]i induced by all agents. The fact that the rise induced by thapsigargin and CPA was reduced indicates that Na/Ca exchanger overexpression provokes a depletion of ER Ca2+ stores.
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DISCUSSION |
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The major observation was that Na/Ca exchanger overexpression led to a reduction in the rise in [Ca2+] i induced by agents stimulating Ca2+ entry into the cell, to a depletion of the ER Ca2+ stores, and to an increase in cell death, whether mediated by Ca2+-dependent or -independent pathways. Cell death appeared to be due to apoptosis as assessed by nuclear DNA staining, DNA laddering, and the quantification of fragmented DNA.
The view that Na/Ca exchanger overexpression would lead to a reduction in the rise in [Ca2+]i induced by agents stimulating Ca2+ entry into the cell was best objectified in the case of tolbutamide. Ionomycin also increases Ca2+ inflow, but may also release Ca2+ from intracellular stores. Interestingly, the initial phase of the increase in [Ca2+] i induced by ionomycin was reduced in overexpressing cells, whereas the late phase was not. The initial phase most probably reflects Ca2+ entry into the cell from the outside instead of Ca2+ release from intracellular stores. Therefore, the data obtained with ionomycin (reduction of the first phase) are consistent with those obtained with the hypoglycemic sulfonylureas. In a previous study, we also showed that the rise in Ca2+ induced by glucose was slightly reduced in Na/Ca exchangeroverexpressing cells compared with control cells (21).
The view that Na/Ca exchanger overexpression led to a depletion of the ER Ca2+ stores is based on the observation that SERCA inhibitors, thapsigargin and CPA, induced a smaller increase in [Ca2+]i in Na/Ca exchangeroverexpressing than in control cells, indicating that the amount of Ca2+ releasable from the ER was reduced in the former cells. The depletion could be directly objectified by the measurement of the ER Ca2+ concentration using furaptra. Both the reduction in [Ca2+] i and the depletion of ER Ca2+ stores can best be understood as the result of an increase in Ca2+ extrusion from the cell. This is consistent with our recent demonstration that Na/Ca exchange contributes to 70% of the extrusion of Ca2+ from rat pancreatic ß-cells (18). In addition, control cells transfected with the vector alone (without the NCX1.7 construct) did not show any difference in thapsigargin- or CPA-induced [Ca2+]i changes compared with nontransfected cells (Figs. 4A and B). Also in agreement with such a view, overexpression of an isoform of the PMCA (2wb) led to similar results, including a reduction in the increase in [Ca2+]i, a depletion in ER Ca2+ stores, and an increased rate of apoptosis (unpublished data). In a previous study, the overexpression of a PMCA in CHO cells also led to a decrease in ER Ca2+ levels (1).
Taken as a whole, these observations indicate that the increased rate of apoptosis observed in overexpressing cells was due to ER Ca2+ depletion. Indeed, apoptosis was increased despite a reduction in the rise in [Ca2+] i, whether SERCA inhibitors or ionomycin were used. Another indication that apoptosis induced by SERCA inhibitors and ionomycin resulted from ER Ca2+ depletion rather than from [Ca2+]i elevation is that the hypoglycemic sulfonylureas, which do not provoke ER Ca2+ depletion, did not induce apoptosis, either in control or overexpressing cells, despite the fact that they increased [Ca2+]i to a similar extent than SERCA inhibitors. Likewise, ionomycin, while provoking a higher increase in [Ca2+]i than in SERCA inhibitors, induced less apoptosis than the latter. Last, the increased rate of apoptosis was accompanied by the activation of caspase-12. Caspase-12, which is localized in the ER, is specifically activated by ER stress, including disruption of ER Ca2+ homeostasis, but not by membrane- or mitochondrial-targeted apoptotic signals (7). Incidentally, our data do not exclude that Na/Ca exchanger overexpression may also lead to a disruption in mitochondrial Ca2+ homeostasis that may also result in apoptosis. Indeed, there are dynamic interactions between ER and mitochondrial Ca2+ stores (32).
Na/Ca exchanger overexpression markedly increased the proapoptotic action of SERCA inhibitors compared with that of ionomycin. This probably is a result of the double action of ionomycin, which permeates both the plasma membrane and the intracellular membranes to Ca2+. By doing so, ionomycin induces a lower release of Ca2+ from the ER because the permeation of the plasma membrane to Ca2+ increases [Ca2+]i, a phenomenon that may counteract ER Ca2+ depletion.
In the current study, one interesting observation was that Na/Ca exchanger overexpression induced caspase-12 activation without increasing the rate of apoptosis. Caspase-12 activation nevertheless sensitized overexpressing cells to apoptotic agents regardless of whether the involved signaling pathway was Ca2+ dependent or independent. This is compatible with the view that caspase-12 is an initiator rather an executor caspase (28).
In a previous study, glucose and hypoglycemic sulfonylureas were shown to induce apoptosis in mouse and rat pancreatic ß-cells (14). Such a phenomenon was not observed in the current study using BRIN-BD11 cells. Although the present study provides no explanation for such a difference, one possibility is that native ß-cells, because they are nontumoral and obtained from islet disruption (e.g., in Ca2+-free medium), are more prone to undergo apoptosis than untreated tumoral cells.
The decrease in cell proliferation appeared to result from the same cause (reduction in ER Ca2+ stores due to increase in Ca2+ outflow) because it could be observed in two clones overexpressing NCX1.7 (current study) and in three clones overexpressing PMCA2wb (unpublished data). This reduction in cell proliferation was not unexpected because Ca2+ is essential for cell growth and survival, although its effects are so widespread that its exact mechanism(s) remain(s) to be completely elucidated (33).
In conclusion, we have shown that Na/Ca exchanger overexpression, by depleting ER Ca2+ stores, triggers the activation of caspase-12 and increases apoptotic cell death by Ca2+-dependent and -independent pathways. Overexpression of the exchanger also led to a decrease in cell proliferation. Because excessive cell proliferation and decreased ability to undergo apoptosis are two hallmarks of cancer or malignancies (4), overexpression of Na/Ca exchanger in cancer cells by gene therapy may represent a new potential approach in cancer therapy. On the other hand, our results also clear a path for the development of new strategies to control cellular Ca2+ homeostasis that could, on the contrary, prevent the process of apoptosis that mediates, in part, ß-cell autoimmune destruction in type 1 diabetes. Indeed, if it is possible to increase apoptosis by overexpressing the Na/Ca exchanger, then it should be possible to reduce it, e.g., by transfecting a Na/Ca exchanger antisense oligonucleotide or by overexpressing a SERCA that may lead to an increase in ER Ca2+ stores.
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ACKNOWLEDGMENTS |
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The authors thank R. Kiss (Laboratoire dHistopathologie) for his help in immunofluorescence microscopy and C. Pastiels and A. Van Praet for their technical help. We also thank P. Vandenabeele (Department of Molecular Biology, Flanders Interuniversity Institute for Biotechnology) and M. Kalai (University of Ghent) for caspase-12 antibodies and for optimizing the Western blot conditions.
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FOOTNOTES |
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Received for publication 20 June 2001 and accepted in revised form 4 March 2002.
[Ca2+]i intracellular calcium concentration; CPA, cyclopiazonic acid; ER, endoplasmic reticulum; MTT, 3-(4,5-dimethylthiazol-2yl)-2,5-diphenyl tetrazolium bromide; PMCA, plasma membrane Ca2+-ATPase; SERCA, sarco(endo)plasmic reticulum Ca2+-ATPase.
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REFERENCES |
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