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The Journal of Neuroscience, May 15, 2000, 20(10):3522-3528
Hypoxia-Induced Silencing of NMDA Receptors in Turtle Neurons
Philip E. Bickler1, Paul H. Donohoe1, 2, and Leslie T. Buck1 Departments of 1 Anesthesia and 2 Neurology, University of California at San Francisco, San Francisco, California 94143
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Hypoxia-induced suppression of NMDA receptors (NMDARs) in western painted turtle (Chrysemys picta) cortical neurons may be critical for surviving months of anoxic dormancy. We report that NMDARs are silenced by at least three different mechanisms operating at different times during anoxia. In pyramidal neurons from cerebrocortex, 1-8 min anoxia suppressed NMDAR activity (Ca2+ influx and open probability) by 50-60%. This rapid decrease in receptor activity was controlled by activation of phosphatase 1 or 2A but was not associated with an increase in [Ca2+]i. However, during 2 hr of anoxia, [Ca2+]i in cerebrocortical neurons increased by 35%, and suppression of NMDARs was predicted by the increase of [Ca2+]i and controlled by calmodulin. An additional mechanism of NMDAR silencing, reversible removal of receptors from the cell membrane, was found in cerebrocortex of turtles remaining anoxic at 3°C for 3-21 d. When suppression of NMDARs was prevented with phosphatase inhibitors, tolerance of anoxia was lost. Silencing of NMDARs is thus critical to the remarkable ability of C. picta to tolerate life without oxygen.
Key words: anoxia; turtles; NMDA receptor; intracellular calcium; phosphatase; receptor downregulation
INTRODUCTION
Typical mammalian neurons are exquisitely sensitive to oxygen deprivation, suffering irreversible injury after brief periods of anoxia. In contrast, western painted turtles (Chrysemys picta) are unusually tolerant of anoxia, surviving 24-48 hr of anoxia at 25°C and 4-5 months at 2-3°C during winter dormancy (Ultsch and Jackson, 1982
). Survival of neurons in these remarkable animals may involve an "arrest" of ion channels that decreases excitability, reduces ion translocation, and preserves [ATP] during the energetic stress imposed by anaerobic conditions (Hochachka, 1986
One of the more striking features of the adaptation of turtle neurons to anoxia is their ability to maintain [Ca2+]i at near normal levels. Excessive Ca2+ influx and Ca2+ toxicity that occurs in anoxic mammalian neurons does not occur in turtle neurons (Bickler, 1998
The regulation of NMDAR activity by phosphorylation of one or more subunits is an important mechanism in the plasticity of glutamatergic synapses (Swope et al., 1999
MATERIALS AND METHODS
These studies were sanctioned by the University of California at San Francisco Committee on Animal Research and conform to relevant National Institutes of Health guidelines for the care of experimental animals. C. picta collected in spring, summer, and autumn were obtained from Lemberger (Oshkosh, WI). The animals were mainly females and weighed 250-650 gm.
All tissue used in these studies was obtained from the cerebrocortex, which is a 1-mm-thick sheet of tissue in this species. After decapitation, the entire brain was removed and placed in oxygenated (95% O2-5% CO2) turtle artificial CSF (aCSF) at 3-5°C (aCSF in mM: 97 NaCl, 26.5 NaHCO3, 2.0 NaH2PO4, 2.6 KCl, 2.5 CaCl2, 2.0 MgCl2, 20 glucose, and 10 HEPES, pH 7.4 at 20°C). Six to eight 3 × 4 mm pieces of cerebrocortex was obtained from each cortex by cutting with fine scissors (Blanton et al., 1989
NMDA receptor function in turtle neurons was assessed with cell-attached patch-clamp recordings and by measuring NMDAR-mediated Ca2+ fluxes (NMDA
Ca2+) with fura-2. Pyramidal neurons used for both patch-clamp recording and [Ca2+]i measurements are located within 50 µm of the ventral surface of the cortical sheets.
Patch-clamp analysis of turtle NMDA receptor open probability. Cell-attached patch-clamp recordings of NMDAR currents and open probability were measured and analyzed as described by Buck and Bickler (1998)
Single-channel NMDAR recordings were made with fire-polished 6-10 M
electrodes containing (in mM): NaCl 115, CsCl 5, CaCl2 2.5, EGTA 10, HEPES acid 10, glycine 0.001, and NMDA 0.01, pH 7.4. Cell-attached 5-20 G
NMDAR activity measured by Ca2+ influx. We also assessed the activity of cortical NMDARs by measuring the increase in [Ca2+]i (NMDA
-conotoxin GIVa, and 0.5 µM agatoxin IVa. In pilot experiments, we found that blocking L-type voltage-gated Ca2+ channels with 1 µM nimodipine or 100 µM Ba2+ did not significantly change measured NMDA
Dissociated neurons from the cerebral cortex were obtained after digestion of cortical sheets with 0.05% trypsin and 0.01% pronase. The tissue was triturated onto coverslips coated with Cell-Tak (Collaborative Research, Bedford MA). Cells were loaded with 2 µM fura-2 AM for 15 min, and then [Ca2+]i changes during NMDA application was measured with a Photon Technology International (Brunswick, NJ) fluorometer system and an inverted microscope (Bickler and Hansen, 1998
Cell viability measurements. Cell viability was assessed by histological appearance of cortical pyramidal neurons in sections of cortical sheets. Sheets were fixed in paraformaldehyde, dehydrated, and embedded in paraffin. They were sectioned (7 µm) and stained with hematoxlyn-eosin and examined with light microscopy. A blinded observer then recorded the percentage of surviving cells in 50 × 100 µm areas. Two of these areas were examined in each slice, and the results were averaged. Dead cells were identified by holes left in the sections, or by cells with grossly altered nuclei or cytoplasm. For comparison, measurements of viability were also made in rat CA1 neurons in hippocampal slices as described previously (Bickler and Hansen, 1998
Trypan blue exclusion was also used as an index of viability in cortical sheets. Tissue was incubated in 0.2% trypan blue for 10 min after an insult and/or recovery. After rinsing in aCSF for 10 min, the presence of blue staining was assessed visually with a dissecting microscope.
ATP concentration was measured with a luciferin-luceriferase assay as described by Buck and Bickler (1995)
NMDAR abundance in membrane fractions from brain cortex homogenates was measured with SDS-PAGE-Western blots. Total protein in the membrane fractions was measured with a standard spectrophotometric assay (Enhanced Protein assay; Pierce, St. Louis, MO), and equal amounts of protein were added to each lane. Immunoblotting to detect turtle NMDARs was done with rat NMDA NR1 antibodies, which reacted strongly with the turtle analog. Primary and secondary antibodies and blocking protein were obtained from Santa Cruz Biotechnology (Santa Cruz, CA). Quantitation of gel staining was done with NIH Image software.
Statistics. Statistical tests were performed using JMP (SAS Institute, Cary, NC). Results in the text and figures are reported as mean ± SE.
RESULTS
Comparative survival of mammalian and turtle neurons during anoxia
To investigate the basis for differences in anoxia sensitivity of turtle and mammalian neurons, we measured membrane potential, ATP levels, trypan blue exclusion, and neuron histology in turtle cortical neurons and rat hippocampal CA1 neurons. In turtle neurons during a 3 hr period of in vitro anoxia (medium bubbled with 95% N2-5% CO2 and containing 1 mM dithionite, PO2 <0.1 mmHg), membrane potential remained stable between
65 and
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Figure 1. Comparison of Chrysemys cerebrocortical neurons and rat CA1 neurons. A, Differences in viability of turtle and rat neurons 5 hr after bouts of anoxia. *p < 0.05 denotes significant difference between turtle and rat groups (ANOVA). B, Anoxia protects turtle neurons from NMDA neurotoxicity, but not when NMDA receptor activity is stimulated with 0.1 nM forskolin or 0.5 µM okadaic acid. *p < 0.05 denotes significant difference from control (Dunnett's test). Numbers above bars indicate number of slices studied, and error bars show 1 SEM.
Is NMDAR silencing critical for cell survival during anoxia?
To examine the coupling between NMDAR function and cell survival or death in turtle neurons, cell survival after exposure to NMDA under oxic (95%O2-5%CO2) and anoxic conditions (95% N2-5% CO2) was measured. In the presence of oxygen, >80% of pyramidal neurons in cortical sheets were killed by exposure to NMDA (100 µM NMDA for 1 hr, wash for 5 hr). With exposure to 200 µM NMDA for 2-4 hr or with 100 µM NMDA and an overnight recovery period, 90-100% of neurons were killed. However, NMDA toxicity was prevented by a 1 hr pretreatment with anoxia, suggesting that anoxia attenuates NMDAR-dependent cell death (Fig. 1B). When the activity of NMDARs was increased by treatment with 0.1 nM forskolin or 0.5 µM okadaic acid (see Figs. 4B, 6C), cell death during anoxia increased significantly. Cell death in anoxic forskolin-treated slices was prevented by 10 µM MK-801. Thus, survival of turtle neurons during anoxia is dependent specifically on reduction in NMDAR-mediated events.
Changes in NMDAR activity during anoxia
The apparent lack of NMDAR-dependent cell death in anoxic turtle neurons led us to test whether NMDARs are suppressed during anoxia and by what mechanisms. To do this, we measured NMDAR activity with patch-clamp electrodes and with fura-2 measurements of NMDA
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Figure 2. Decrease in NMDA receptor activity during anoxia. A, Decrease in mean NMDA receptor open probability in cell-attached patches during 90 min of anoxia. Patch pipettes contained 10 µM NMDA. *p < 0.05 denotes significant decrease compared with normoxic control (Dunnett's test). Error bars show 1 SEM; n = 6-8 for each data point. B, Examples of [Ca2+]i changes produced by 100 µM NMDA (arrows) in cortical sheets in normoxic and anoxic conditions and after recovery from anoxia. C, Mean NMDA receptor activity (NMDA
During 2 hr of anoxia, the amplitude of NMDA
Changes in NMDAR activity and abundance during anoxia
We next investigated whether a decrease in the number of receptors present in the membrane of neurons might account for part of the decrease in NMDA
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Figure 3. Changing abundance of NMDA receptors during anoxia and recovery. Top portion shows representative Western immunoblots of NR1 NMDA subunits. Bottom graph shows changes in receptor abundance during 3 hr to 3 weeks of anoxia (submergence in 3°C anoxic water) and recovery.
Role of receptor phosphorylation control in NMDAR silencing
To test whether phosphorylation control participates in NMDAR silencing during anoxia, we exposed isolated neurons to the nonspecific phosphatase inhibitor okadaic acid. We found that low concentrations of okadaic acid (120 nM) prevented the anoxia-induced suppression of NMDA
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Figure 4. Role of phosphatases in the regulation of NMDA receptors during anoxia. A, Example showing that the nonspecific phosphatase inhibitor okadaic acid prevents NMDA receptor inactivation in a dissociated pyramidal neuron during anoxia. B, Phosphatase inhibitors prevent receptor silencing in cortical sheets during anoxia. Bars show mean NMDA
Role of Ca2+ in NMDAR regulation during anoxia
During 2 hr of anoxia, [Ca2+]i in neurons in cortical sheets increased from 135 ± 6 to 202 ± 5 nM (n = 6, p < 0.001) (Fig. 5A). This increase in [Ca2+]i predicted the depression NMDAR activity during anoxia (regression significant, p < 0.01). NMDAR activity was predicted by [Ca2+]i during oxic conditions as well (Fig. 5B).
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Figure 5. [Ca2+]i predicts NMDA receptor activity in both oxic and anoxic neurons in cortical sheets. A, Two hours of in vitro anoxia increased [Ca2+]i by 32% (70 nM). B, Significant correlation of [Ca2+]i to NMDA receptor activity in both oxic or anoxic neurons. Lines show least-squares linear regression for each group of neurons.
We examined whether the calcium-dependent signaling protein calmodulin participates in NMDAR regulation during anoxia. Calmidazolium, an inhibitor of calmodulin, decreased NMDAR activity ~38% in the presence of oxygen, suggesting that calmodulin normally acts as a positive modulator of NMDAR activity. During anoxia, calmidazolium prevented a further decrease in NMDAR activity, suggesting that calmodulin, or another signaling molecule associated with it, normally plays some role in the inactivation of receptor function (Fig. 6A). We also investigated whether the calcium-calmodulin-dependent phosphatase calcineurin (phosphatase 2B) plays a role in suppressing NMDAR function. Cypermethrin, a specific calcineurin inhibitor, was used. We found that calcineurin inhibition produced a slight, nonsignificant decrease in NMDAR activity in both aerobic and anaerobic conditions. However, cypermethrin did not prevent anoxia from suppressing NMDAR activity, suggesting that activation of calcineurin does not contribute to the inactivation of NMDARs during anaerobic conditions (Fig. 6B).
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Figure 6. Regulation of NMDA receptor activity during anoxia by Ca2+-dependent processes. A, Inhibition of the Ca2+ binding protein calmodulin reduced NMDA receptor silencing during anoxia. Cortical sheets were treated with 10 nM calmidazolium 30 min before and during 2 hr anoxia or with O2 present. NMDA
Protein kinase A (PKA) is an important regulator of NMDARs under aerobic conditions (Swope et al., 1999
DISCUSSION
Importance of NMDA receptor silencing to surviving anoxia
We have shown that the silencing of NMDARs in anoxic turtle neurons occurs by at least three mechanisms of different time courses. Suppression of receptors within minutes of anoxia is controlled by protein phosphorylation. During several hours of anoxia, receptors are silenced by processes related to elevated [Ca2+]i, whereas over days to weeks of oxygen deprivation, receptors are removed from the cell membrane. These different controls achieve depression of NMDAR function that may enable turtle neurons to survive the energetic challenge of prolonged oxygen deprivation that accompanies diving or winter dormancy. Energy expenditure in anoxic turtle tissues is reduced by 90-99% (Buck and Hochachka, 1993
Mechanisms of NMDAR regulation during anoxia
During the first few minutes of anoxia, the turtle NMDAR is inactivated by a mechanism involving phosphatase 1 or 2A. These phosphatases decrease the activity of mammalian NMDARs and may play important roles in the long-term control of glutamatergic synapses (Mulkey et al., 1993
The activity of NMDARs in turtle neurons was influenced by cAMP-protein kinase A, similar to mammalian receptors (Swope et al., 1999
Dephosphorylation of NMDARs by phosphatases early in anoxia may be related to later changes in NMDAR expression or distribution. We speculate that dephosphorylation tags inactive NMDARs for internalization at a later time. Receptor internalization-redistribution may be a common phenomenon controlling receptor function. It has been described for metabotropic glutamate receptors (Doherty et al., 1999
Role of Ca2+ in NMDAR regulation
In turtle neurons, [Ca2+]i increases ~30% above basal during 2 hr of anoxia. This increase, which remains stable through 6 weeks of anoxia (Bickler, 1998
Calcium-dependent depolymerization of the cytoskeleton is responsible for NMDAR desensitization, which occurs when [Ca2+]i reaches high levels (Rosenmund and Westbrook, 1993
We have not ruled out the contribution of other possible controls of NMDAR function during anoxia. Adenosine, which accumulates in the extracellular space during anoxia, has been shown to contribute to NMDAR suppression (Buck and Bickler, 1998
Turtle neurons as models for identifying new neuroprotection strategies
The present study offers several insights into the role of glutamate receptors and [Ca2+]i in determining neuron survival during anoxia. Turtle neurons survive anoxia by suppressing NMDAR function, which is not surprising in view of the protective qualities of NMDAR antagonists in mammalian brain ischemia (Lee et al., 1999
FOOTNOTES Received Dec. 6, 1999; revised Feb. 1, 2000; accepted Feb. 11, 2000.
This work was supported by National Institutes of Health Grants R29 GMS 55212 (P.E.B.) and PO1 NS 35902 (P.H.D.). We thank Bonnie Hansen, Melanie Vose, Rick Liniger, and Breandan Sullivan for technical support.
Correspondence should be addressed to Dr. Philip Bickler, Department of Anesthesia, Sciences 261, University of California at San Francisco, 513 Parnassus Avenue, San Francisco, CA 94143-0542. Email: bicklerp{at}anesthesia.ucsf.edu.
Dr. Donohoe's present address: National Institute of Medical Research, London, UK NW7 1AA.
Dr. Buck's present address: Department of Zoology, University of Toronto, Toronto, Ontario, Canada M5S 3G5.
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Copyright © 2000 Society for Neuroscience 0270-6474/00/20103522-07$05.00/0
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