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The Journal of Neuroscience, June 1, 2003, 23(11):4737-4745
Previous Article | Next Article
Transient Receptor Potential Channel Activation Causes a Novel Form of [Ca 2+]i Oscillations and Is Not Involved in Capacitative Ca 2+ Entry in Glial Cells
Maurizio Grimaldi, Marina Maratos, andAjay Verma Department of Neurology, Uniformed Services University of the Health Sciences, Bethesda, Maryland 20814
Abstract
Top
Abstract
Introduction
Astrocytes express transient receptor potential channels (TRPCs), which have been implicated in Ca 2+ influx triggered by intracellular Ca 2+ stores depletion, a phenomenon known as capacitative Ca 2+ entry. We studied the properties of capacitative Ca 2+ entry in astrocytes by means of single-cell Ca 2+ imaging with the aim of understanding the involvement of TRPCs in this function. We found that, in astrocytes, capacitative Ca 2+ entry is not attributable to TRPC opening because the TRPC-permeable ions Sr2+ and Ba2+ do not enter astrocytes during capacitative Ca 2+ entry. Instead, natively expressed oleyl-acetyl-glycerol (OAG) (a structural analog of DAG) -sensitive TRPCs, when activated, initiate oscillations of cytosolic Ca 2+ concentration ([Ca 2+]i) pharmacologically and molecularly consistent with TRPC3 activation. OAG-induced [Ca 2+]i oscillations are not affected by inhibition of inositol trisphosphate (InsP3) production or blockade of the InsP3 receptor, therefore representing a novel form of [Ca 2+]i signaling. Instead, high [Ca 2+]i inhibited oscillations, by closing the OAG-sensitive channel. Also, treatment of astrocytes with antisense against TRPC3 caused a consistent decrease of the cells responding to OAG. Exogenous OAG but not endogenous DAG seems to activate TRPC3. In conclusion, in glial cells, natively expressed TRPC3s mediates a novel form of Ca 2+ signaling, distinct from capacitative Ca 2+ entry, which suggests a specific signaling function for this channel in glial cells.
Key words: astrocyte; transient receptor potential channel; store-operated Ca 2+ channels; [Ca 2+]i oscillations; capacitative Ca 2+ entry; C6 glioma cells
Introduction
Since the original description of Ca 2+ entry triggered by depletion of intracellular Ca 2+ stores (Putney, 1986), progress has been slow to identify the plasma-membrane channels involved in this phenomenon. Transient receptor potential channels (TRPCs), a family of relatively nonselective divalent cation channels, have been proposed as the molecular entity associated with store-operated Ca 2+ channel activity (Zhu et al., 1996
Little is known about capacitative Ca 2+ entry, store-operated Ca 2+ channels, or TRPC function in the Ca 2+ homeostasis of type I astrocytes. In this study, we analyzed the properties and the behavior of capacitative Ca 2+ entry in type I astrocytes and C6 glioma cells, with the aim of clarifying the role of natively expressed TRPCs in this phenomenon. We were able to pharmacologically distinguish store-operated Ca 2+ channel function from TRPC activity. Furthermore, we identified a possible role for oleyl-acetyl-glycerol (OAG)-sensitive TRPC activation in the generation of a novel form of astrocytic [Ca 2+]i oscillations.
Materials and Methods
Cell cultures. Type I astrocyte cultures were obtained from embryonic day 17 rats according to a published protocol (Grimaldi et al., 1994Single cell [Ca 2+]i measurements. Nearly confluent type I astrocytes and C6 glioma cells were seeded onto 1.5-cm-diameter glass coverslips (Assistent, Sondheim/Rhön, Germany). Before the experiment, cells were washed once in Krebs'–Ringer's buffer (KRB) containing the following (in mM): 125 NaCl, 5 KCl, 1 Na2HPO4, 1 MgSO4, 1 CaCl2 1, 5.5 glucose, and 20 HEPES, pH 7.3. They were then loaded with 4 µM fura-2 AM (Molecular Probes, Eugene, OR) for 22 min at room temperature under continuous gentle agitation. After loading, cells were washed once with fresh KRB and then incubated for an additional 22 min in KRB without fura-2 AM, according to a previously published protocol (Grimaldi et al., 1999
800 µl/min. Ca 2+-free solutions were prepared by omitting Ca 2+ from the KRB and including 100 µM EGTA. Ratio measurements were performed every 2 sec by collecting image pairs exciting the preparations at 340 and 380 nm, respectively. The excitation wavelengths were changed through a high-speed mechanical filter changer, and the emission wavelength was set at 510 nm. The captured images were digitized using an acquisition board and analyzed by using commercially available software. Ratio values were derived from the entire cytosolic area, obtained by delimiting the profile of the cells and averaging the signal within the delimited area, and were converted into [Ca 2+]i using the equation described by Grynkiewicz et al. (1985
Reverse transcription-PCR. Primers to the six isoforms of TRPC1–TRPC6 and to
-actin were designed according to published sequences (Pizzo et al., 2001
Antisense oligonucleotides were designed on the basis of the sequence specificity. We synthesized an antisense on the basis of the primers used for the PCR, specific for the isoform TRPC3. We also synthesized fluoresceinate antisense, sense, and scrambled oligonucleotides. Astrocytes were treated with 100 µg/ml antisense, sense, or scrambled oligonucleotides and with fluoresceinate antisense to control for uptake. After
Western blot. Proteins were extracted from type I astrocytes and C6 glioma cells using the Protease Arrest kit (Geno Technology, St. Louis, MO). Protein content of the samples was quantified using the Bradford assay (Bradford, 1976
Immunocytochemistry and confocal analysis of TRPC3 and TRPC4 localization. Type I astrocytes and C6 cells seeded on coverslips were fixed in 4% paraformaldehyde in PBS. Cells were incubated with primary antibody to TRPC3 and TRPC4, at 1:25 dilution, for 4 hr at room temperature (Alomone Labs). Preparations were washed several times in PBS. Secondary FITC-conjugated antibody at 1:200 dilution was incubated for 1 hr at room temperature. Preparations were washed several times in PBS. Coverslips were mounted using Immunomount containing the antifade agent DABCO (1,4-diazabicyclo-[2.2.2]octane). Preparations were observed with an inverted microscope using 40x oil immersion high numerical aperture Olympus Optical (Tokyo, Japan) lens. Images were enlarged using the optical zoom of the microscope; therefore, final magnification was 60x. Images were digitized using commercially available software.
Materials. All materials were purchased from Sigma (St. Louis, MO), unless otherwise specified in the text.
Use of laboratory animals. Adequate measures were taken to minimize unnecessary pain and discomfort to the animals and to minimize animal use according to NIH Guide for the Care and Use of Laboratory Animals. Pregnant animals were killed by exposure to CO2 according to approved protocols.
Statistical analyses. Experiments were performed at least three times on different cell preparations. For [Ca 2+]i measurements, digital images were converted to analog data and imported to a spreadsheet. The numbers generated, representing the [Ca 2+]i determined every 2 sec, were averaged and SEs were calculated. Plots represent the average ± SE of all of the cells studied. In studies on [Ca 2+]i oscillations, graphs display representative cells, and frequency analysis of the population is displayed in an associated bar graph. When statistical validation was required, the values of the specified data points were analyzed by ANOVA, followed by Student's t test and shown as a bar inset. Differences were considered statistically significant when the p < 0.05. For experiments based on all-or-none responses, such as the one on the percentage of responding cells, a different statistical analysis was performed using the Wilcoxon ranked test, which allows determining statistical significance in this type of response.
Results
Store-operated Ca 2+ channels in type I astrocytes and in C6 cells do not exhibit TRPC properties
We depleted intracellular Ca 2+ stores by exposure to 2 µM thapsigargin, an irreversible inhibitor of the sarcoendoplasmic reticulum Ca 2+ ATPase (SERCA) (Thastrup et al., 1989
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Figure 1. Depletion of intracellular Ca 2+ stores achieved via exposure to thapsigargin is not associated with the opening of TRPC.A,D, Astrocytes and C6 were exposed to 2 µM thapsigargin (Thap) in the absence of extracellular Ca 2+ to deplete intracellular Ca 2+ stores, after which cells were reperfused with 1 mM extracellular Ca 2+ to initiate capacitative Ca 2+ entry. In both celltypes, initiation of capacitative Ca 2+entry generated a consistent elevation of[Ca 2+]ithat was larger in C6 than in astrocytes. B, E, Astrocytes and C6, respectively, were exposed to 2 µM thapsigargin. When intracellular Ca 2+ stores depletion was complete, 1 mM Sr 2+ was introduced in the extracellular solution. In both astrocytes and C6, very little Sr 2+ entered the cells during capacitative Ca 2+ entry. Successively, Sr 2+ was replaced with Ca 2+ to check that capacitative Ca 2+ entry was still activated in this condition. C, F, Astrocytes and C6, respectively, were exposed to 2 µM thapsigargin in the presence of 1 mM extracellular Ca 2+. When [Ca 2+]i elevation reached a plateau and stabilized, extracellular Ca 2+ was replaced by 1 mM Sr 2+. Capacitative Ca 2+ entry was promptly terminated, indicating that Sr 2+ is an antagonist of the store-operated Ca 2+ channels (note that, to ease readability, values are reported as calibrated Ca 2+ values even when Sr 2+ is present).
Store-operated Ca 2+ channels are highly selective (Hoth and Penner, 1992
We also depleted intracellular Ca 2+ stores with ATP, a purinergic P2y receptor agonist that induces the production of the second messengers InsP3 and DAG (Shao and McCarthy, 1993
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Figure 2. Depletion of intracellular Ca 2+ stores induced by InsP3-elevating agents is not associated with the opening of TRPC. A, B, Astrocytes and C6 cells, respectively, were challenged with ATP in the absence of extracellular Ca 2+ until intracellular Ca 2+ stores were emptied, as testified by the return to baseline of [Ca 2+]i. Next, 1 mM Sr 2+ was supplied in the extracellular solution. Sr 2+ did not enter the cells, indicating that intracellular Ca 2+ stores depletion induced by the ATP was not associated with TRPC opening (note that, to ease readability, values are reported as calibrated Ca 2+ values even when Sr 2+ is present).
Astrocytes and C6 glioma cells differentially express TRPCs
Using RT-PCR, we showed that astrocytes express mRNA for all six TRPC subtypes (Fig. 3A) (Pizzo et al., 2001
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Figure 3. Expression of TRPC in astrocytes and C6 glioma cells. A, mRNA extracted from astrocytes was amplified with primers designed to amplify TRPC1–TRPC6 and
OAG activation of TRPCs induces high-amplitude, low-frequency [Ca 2+]i oscillations
Several studies have reported that OAG causes the opening of TRPC3 and TRPC6 and in some instances of TRPC1, independent of lipid-sensitive protein kinase C activation (Hofmann et al., 1999
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Figure 4. Effect of activation of OAG-sensitive TRPC in astrocytes and C6 glioma cells. A, Exposure to 100 µM OAG evoked low-frequency, high-amplitude [Ca 2+]i oscillations after a brief delay. B, [Ca 2+]i oscillations were not affected when extracellular Ca 2+ was exchanged with Sr 2+, suggesting that they were attributable to activation of TRPC. C, Exposure of astrocytes to 100 µM OAG in the absence of extracellular Ca 2+ failed to cause oscillations. D, Percentage of astrocytes responding to OAG with [Ca 2+]i oscillations. Vehicle astrocytes (black bar), OAG-treated cells in the presence of 1 mM extracellular Ca 2+(white bar), 1 mMSr2+(gray bar), or 0 extracellular Ca 2+(hatched bar) in the extracellular solution.E, Exposure of C6 cells to 100 µM OAG evoked low-frequency, high-amplitude[Ca 2+]ioscillations.F, Also in C6 cells,[Ca 2+]ioscillations were not inhibited when extracellular Ca 2+was exchanged with Sr2+, suggesting that they were attributable to activation of TRPC. G, Exposure of C6 glioma cells to 100 µM OAG in the absence of extracellular Ca 2+ failed to cause oscillations. H, Percentage of C6 cells responding to OAG with [Ca 2+]i oscillations. Vehicle-treated cells (black bar), OAG-treated cells in the presence of 1 mM extracellular Ca 2+ (white bar), 1 mM Sr2+ (gray bar), or 0 extracellular Ca 2+ (hatched bar) in the extracellular solution. ** indicated a statistically significant difference versus control cells as assessed by Wilcoxon ranked test (note that, to ease readability, values are reported as calibrated Ca 2+ values even when Sr2+ is present).
OAG-induced [Ca 2+]i oscillations were maintained in extracellular solution containing 1 mM Sr2+ and no Ca 2+, indicating that they were, attributable to the opening of a nonselective cation channel, likely a TRPC (Fig. 4B,F). [Ca 2+]i oscillations are believed to be attributable to either cyclical release of InsP3 and/or Ca 2+-mediated desensitization and subsequent resensitization of the InsP3 receptor (Hajnoczky and Thomas, 1997
Treatment of astrocytes with an antisense (100 µg/ml) designed to inhibit the expression of TRPC3 greatly reduced the percentage of astrocytes responding to OAG (Fig. 5). Approximately 99% of the astrocytes treated with vehicle (n = 154; r = 3) or sense sequence (n = 130; r = 3) responded to OAG exposure with [Ca 2+]i oscillations as untreated cells. Only
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Figure 5. Effect of anti-TRPC3 antisense oligonucleotides on OAG-induced [Ca 2+]i oscillations. Astrocytes were treated for 36 hr with vehicle, and 100 µg/ml TRPC3 sense or antisense oligonucleotides were loaded with fura-2 and then exposed to 100 µM OAG. Open bars indicate responding cells, and filled bars indicate nonresponding cells. Anti-TRPC3 oligunucleotide treatment significantly reduced the number of astrocytes (AS) responding to OAG. Statistical analysis was performed with Wilcoxon ranked test. * indicates a significant difference versus vehicle.
Regulation of OAG-induced [Ca 2+]i oscillations
We studied OAG-triggered [Ca 2+]i oscillations under conditions affecting InsP3 production.Pretreatment with phorbol esters has been shown to inhibit both phospholipase C (PLC) activity (Chuprun and Rapoport, 1997
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Figure 6. Inhibition of InsP3-mediated Ca 2+ mobilization does not affect OAG-induced [Ca 2+]i oscillations in type I astrocytes. A, Astrocytes exposed to 10 µM ATP respond with a typicalCa 2+transient response characterized by a fast, large initialrise, followed by a sustained [Ca 2+]i elevation phase to a lower [Ca 2+]i. B, Astrocytes treated with 10 µM PMA (solid horizontal bar) showed a severely inhibited response to ATP. C, 2-APB at 80 µM, a blocker of the InsP3 receptor, almost completely blocked the effect of ATP on [Ca 2+]i. D, Preexposure of astrocytes to PMA did not affect the appearance or the amplitude of OAG-induced [Ca 2+]i oscillations. E, Pretreatment with 80 µM 2-APB failed to affect OAG-induced [Ca 2+]i oscillations. F, Pretreatment of astrocytes with 10 µM OAG did not trigger [Ca 2+]i oscillations but also did not affect the ability of 100 µM OAG to trigger [Ca 2+]i oscillations.
We next asked whether [Ca 2+]i could regulate the activity of the OAG-sensitive TRPC. We used different experimental approaches to elevate [Ca 2+]i to different levels and assessed the function of OAG-activated TRPC. ATP exposure was not able to trigger [Ca 2+]i oscillations (Fig. 7A), nor did it affect OAG-induced [Ca 2+]i oscillations (Fig. 7B). However, OAG-induced [Ca 2+]i oscillations in the presence of ATP were completely prevented by extracellular Ca 2+ withdrawal, whereas ATP response was completely preserved (Fig. 7B, inset). The [Ca 2+]i transient evoked by ATP is characterized by a rapid peak, followed by a prolonged plateau phase at a lower [Ca 2+]i. The latter could not be high enough to affect TRPCs. Therefore, we evaluated the effect of a more prolonged and marked [Ca 2+]i elevation. Thapsigargin causes a prolonged elevation of [Ca 2+]i and avoids reuptake in the intracellular Ca 2+ stores (Fig. 8A). In the presence of thapsigargin and extracellular Ca 2+, OAG-triggered [Ca 2+]i oscillations were still observed. The increasingly higher [Ca 2+]i reached after each oscillation was attributable to the inability of the thapsigargin-treated cells to take up Ca 2+ in the intracellular Ca 2+ stores (Fig. 8B). OAG-induced [Ca 2+]i oscillations in the presence of thapsigargin were preserved in the presence of extracellular Sr2+, indicating that TRPC can still be activated in this condition (Fig. 8D). Additionally, this set of experiments indicates that TRPC opening is not potentiated by intracellular Ca 2+ stores depletion, contrary to what one would expect, if TRPC was being operated by intracellular Ca 2+ stores depletion (Fig. 8B).
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Figure 7. Preexposure to an agonist mobilizing Ca 2+ from intracellular Ca 2+ stores does not affect OAG-triggered [Ca 2+]i oscillations. A, Exposure of astrocytes to ATP causes a typical [Ca 2+]i transient response characterized by a peak followed by much lower plateau phase. B, Astrocytes were exposed simultaneously to ATP and OAG. The ability of OAG to initiate [Ca 2+]i oscillations during the plateau phase of the ATP response was completely unaffected. The inset in B shows that, although the peak phase of the response to ATP is preserved in the absence of extracellular Ca 2+, both the plateau phase of the ATP response and OAG-induced [Ca 2+]i oscillations are prevented by removal of extracellular Ca 2+.
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Figure 8. Exposure to thapsigargin does not affect OAG-induced [Ca 2+]i oscillations in astrocytes. A, Treatment with 2 µM thapsigargin (Thap) elevates [Ca 2+]i. B, Astrocytes were exposed simultaneously to thapsigargin and 100 µM OAG. Depletion of intracellular Ca 2+ stores and mild [Ca 2+]i elevation of did not affect OAG-evoked [Ca 2+]i oscillations. C, When extracellular Ca 2+ is exchanged with 1 mM Sr 2+, 2 µM thapsigargin elevated [Ca 2+]i, but the prolonged plateau phase was lost. D, Effect of 2 µM thapsigargin and 100 µM OAG in the presence of 1 mM extracellular Sr 2+. OAG is still able to induce[Ca 2+]ioscillations(note that, to ease readability, values are reported as calibrated Ca 2+ values even when Sr 2+ is present).
Whereas ATP and thapsigargin individually do not affect OAG-induced [Ca 2+]i oscillations, the simultaneous exposure to ATP and thapsigargin caused a high, long-lasting [Ca 2+]i elevation (Fig. 9A) and completely prevented OAG-induced oscillations. This suggests that a large [Ca 2+]i elevation may block OAG-sensitive TRPC function (Fig. 9A vs B). To assess whether, in the presence of ATP, thapsigargin, and OAG, the OAG-sensitive TRPCs are open and only the oscillatory activity is lost, we exposed the cells to ATP–thapsigarin–OAG in the presence of extracellular Sr2+. Stimulation of astrocytes with ATP and thapsigargin did not result in any Sr2+ entry (Fig. 9C). When astrocytes were exposed to ATP–thapsigargin–OAG, again no Sr2+ influx was recorded, suggesting that, after a large [Ca 2+]i elevation, as achieved with the simultaneous exposure to ATP and thapsigargin, the OAG-sensitive TRPC is closed (Fig. 9C vs D). We performed an additional experiment using Ba2+, which is also conducted by OAG-sensitive TRPCs, but is not pumped into the endoplasmic reticulum by SERCA (Vanderkooi and Martonosi, 1971
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Figure 9. Effect of high [Ca 2+]i on OAG-induced oscillations: A, We induced a large and persistent elevation of [Ca 2+]i by challenging astrocytes with both 10 µM ATP and 2 µM thapsigargin (Thap). B, Under this condition, OAG failed to cause [Ca 2+]i oscillations. C, In the presence of ATP and thapsigargin, there was no influx of Sr 2+, suggesting TRPC channel closure. D, Astrocytes were exposed to ATP, thapsigargin, and OAG simultaneously in the presence of 1 mM extracellular Sr 2+. In this condition, no Sr 2+ entry was detected. Extracellular Ca 2+ solution at 1 mM was then added and a large[Ca 2+]ielevation was detected, indicating a strong capacitative Ca 2+ entry activation (note that, to ease readability, values are reported as calibrated Ca 2+ values even when Sr 2+ is present).
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Figure 10. Effect of OAG in the presence of the large divalent cation Ba 2+. Astrocytes were perfused with 1 mM Ba 2+ and 0 Ca 2+. Cells were then exposed to 100 µM OAG, which caused a gradual and large elevation of fura-2 ratio signal (R340/380).
[Ca 2+]i oscillations are not mimicked by endogenous DAG elevation
We conducted experiments designed to test whether endogenous DAG can trigger [Ca 2+]i oscillations similar to exogenously applied OAG. In other cells in which TRPCs were overexpressed, inhibition of DAG-lipase by RHC80276 activates TRPC channels, presumably via the accumulation of basally released and uncatabolized DAG (Hofmann et al., 1999
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Figure 11. Effect of DAG-lipase blockade on [Ca 2+]i in un stimulated and ATP-stimulated astrocytes. A, Astrocytes were perfused with the compound RHC80276. The agent did not cause any change of[Ca 2+]i.B, RHC80276 did not affect[Ca 2+]ielevation induced by 10 µMATP, nor were oscillations observed.
Discussion
Capacitative Ca 2+ entry is a well known phenomenon occurring in a wide variety of cell types. Capacitative Ca 2+ entry provides Ca 2+ for intracellular Ca 2+ stores refilling and to sustain prolonged [Ca 2+]i elevations in response to InsP3-linked agonists. We and others have shown in astrocytes that Ca 2+ entry is activated in response to intracellular Ca 2+ stores depletion and that capacitative Ca 2+ entry participates in regulating the magnitude of responses to Ca 2+-mobilizing agonists (Grimaldi et al., 1999Several isoforms of TRPC are expressed in type I astrocytes (Pizzo et al., 2001
[Ca 2+]i oscillations have been observed in some cell types, including astrocytes (Berridge, 1990
It is commonly believed that the second messenger operating the TRPC3 channels is DAG (Hofmann et al., 1999
In conclusion, we determined that store-operated Ca 2+ channels activity is not mediated by TRPC opening in glial cells. We also identified a potentially novel mode of Ca 2+ signaling in glial cells attributable to the activation of TRPC3. This novel mode of Ca 2+ signaling takes the form of high-amplitude [Ca 2+]i oscillations repeating at low frequency that is independent of InsP3 and mobilization of intracellularly stored Ca 2+, hence differing from previously described oscillatory phenomenon. These [Ca 2+]i oscillations are blocked by high [Ca 2+]i and may be induced by an extracellular congener of DAG, released by nearby neurons or astrocytes. We propose that such a signaling pathway may play a relevant role in glial physiology.
Footnotes
Received Dec. 2, 2002; revised Mar. 12, 2003; accepted Mar. 12, 2003.This work was supported by Department of Defense Grants MDA905-02-2-0001 and MDA905-001-034 and National Institutes of Health Grant 5 RO1 NS37814 (A.V.). We gratefully acknowledge Dr. Laurel Haak for her critical discussion of the data and for her help in editing this manuscript.
Correspondence should be addressed to Dr. Maurizio Grimaldi, Department of Neurology, Uniformed Services University of the Health Sciences, Room B3007, 4301 Jones Bridge Road, Bethesda, MD 20814. E-mail: mgrimaldi{at}usuhs.mil.
Copyright © 2003 Society for Neuroscience 0270-6474/03/234737-09$15.00/0
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