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Cannabinoids And Neuroprotection In Global And Focal Cerebral Ischemia

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Abstract

Marijuana and related drugs (cannabinoids) have been proposed as treatments for a widening spectrum of medical disorders.R(+)-[2,3-dihydro-5-methyl-3-[(morpholinyl)methyl]pyrrolo[1,2,3-de]-1,4-benzoxazin-yl]-(1-naphthalenyl)methanone mesylate (R(+)-WIN 55212-2), a synthetic cannabinoid agonist, decreased hippocampal neuronal loss after transient global cerebral ischemia and reduced infarct volume after permanent focal cerebral ischemia induced by middle cerebral artery occlusion in rats. The less active enantiomerS(−)-WIN 55212-3 was ineffective, and the protective effect of R(+)-WIN 55212-2 was blocked by the specific central cannabinoid (CB1) cannabinoid receptor antagonistN-(piperidin-1-yl)-5-(4-chlorophenyl)-1-(2,4-dichlorophenyl)-4-methyl-1H-pyrazole-3-carboxamide-hydrochloride.R(+)-WIN 55212-2 also protected cultured cerebral cortical neurons from in vitro hypoxia and glucose deprivation, but in contrast to the receptor-mediated neuroprotection observed in vivo, this in vitro effect was not stereoselective and was insensitive to CB1 and CB2 receptor antagonists. Cannabinoids may have therapeutic potential in disorders resulting from cerebral ischemia, including stroke, and may protect neurons from injury through a variety of mechanisms.

Introduction

Cannabis, the marijuana plant, has been used since antiquity for its medicinal and psychoactive properties (Snyder, 1971). Both its principal active ingredient, Δ9-tetrahydrocannabinol (THC), and synthetic analogs thereof (cannabinoids) have been proposed as therapy for a variety of medical conditions, including glaucoma, cancer chemotherapy-induced nausea and vomiting, acquired immunodeficiency syndrome, inflammatory disorders, and epilepsy (Jack, 1997). This has contributed to efforts to legalize marijuana use for therapeutic purposes (Annas, 1997; Kassirer, 1997). However, concern exists about the safety of cannabinoids, including their possible role in infertility (Schmid et al., 1997) and the extent to which they share effects with narcotics (Rodrı́guez de Fonseca et al., 1997; Tanda et al., 1997). This controversy persists despite major advances regarding the basic molecular and cellular mechanisms of cannabinoid action (for review, see Felder and Glass, 1998), including the discovery of endogenous cannabinoids (Devane et al., 1992; Stella et al., 1997; Randall and Kendall, 1998), mechanisms for their synthesis and termination of action (Di Marzo et al., 1994; Beltramo et al., 1997), cannabinoid receptors (Matsuda et al., 1990; Kuster et al., 1993; Howlett, 1995), receptor—effector coupling pathways (Mackie and Hille, 1992;Derkinderen et al., 1996), and synthetic cannabinoid agonist and antagonist drugs (Compton et al., 1992; Rinaldi-Carmona et al., 1994).

Central cannabinoid (CB1) receptors are coupled to several signal transduction pathways, including G-proteins that inhibit N-type voltage-gated calcium channels involved in the release of neurotransmitters (Mackie and Hille, 1992). These channels participate in release of the excitatory transmitter L-glutamate, which has been implicated in the death of neurons from stroke, hypoxia, hypoglycemia, and epilepsy. In hippocampal cultures, cannabinoid agonists acting through CB1 receptors and G-proteins inhibit glutamate release (Shen et al., 1996), suggesting that they might reduce glutamate-mediated neuronal injury. Therefore, we examined the effect of cannabinoids on neuronal death in the selectively vulnerable CA1 region of rat hippocampus after transient global cerebral ischemia induced by four-vessel occlusion, on infarct volume after permanent occlusion of the middle cerebral artery (MCA) and on the viability of cultured cerebral cortical neurons deprived of oxygen and glucose in vitro.

MATERIALS AND METHODS

Animals. Animal experiments were approved by local committee review and were conducted according to policies on the use of animals of the Society for Neuroscience. Male Sprague Dawley rats weighing 300—330 gm (global ischemia studies) or 280—310 gm (focal ischemia studies) were used. Anesthesia was induced with 4% isoflurane, 66% N2O, and 30% O2 and, after intubation, maintained with 1.5% isoflurane, 68.5% N2O, and 30% O2. The left femoral artery was cannulated to monitor arterial blood pressure, blood gases, and blood glucose concentration. Rectal temperature was monitored continuously and maintained at 37.0—37.5°C using a heating pad. In global ischemia studies, brain temperature was monitored with a 29 gauge thermocouple implanted in the right striatum and was maintained at 36—37°C with a temperature-regulated heating lamp. In focal ischemia studies, the temperature of the temporalis muscle contralateral to MCA occlusion was monitored and maintained at 37.0—37.5°C in the same manner.

Global cerebral ischemia. Global cerebral ischemia lasting 15 min, followed by reperfusion, was induced by four-vessel occlusion in anesthetized rats (Pulsinelli et al., 1982). Animals were placed in a Kopf stereotactic frame, and the vertebral arteries were coagulated and transected at the junction of the C1 and C2 vertebrae under microscopic guidance. The common carotid arteries (CCAs) were then exposed, the external carotid arteries (ECAs) were ligated, and administration of isoflurane was discontinued. Three minutes later, the CCAs were occluded reversibly for 15 min with microvascular clips, and perfusion was then restored. The electroencephalogram was monitored to ensure isoelectricity during the period of ischemia. Temperature was monitored from the time of intubation until ∼30 min after the onset of reperfusion, for a total of ∼50—70 min.

Focal cerebral ischemia. Permanent focal ischemia was induced by intraluminal occlusion of the MCA with a suture (Longa et al., 1989). Under a microscope, the left ECA was ligated with a 6-0 silk suture and dissected distally, and the left internal carotid artery (ICA) was isolated and separated from the vagus nerve. The extracranial branch of the left ICA was ligated close to its origin with a 6-0 silk suture. A 3-0 surgical monofilament nylon suture with a rounded tip was introduced into the left ICA lumen through the stump of the left ECA and advanced 20—21 mm past the CCA bifurcation. The suture was left in place until rats were killed 24 hr after the onset of ischemia. Temperature was monitored from the time of intubation until ∼30 min after the onset of ischemia, for a total of ∼30—45 min.

Drug administration. R(+)-[2,3-dihydro-5-methyl-3-[(morpholinyl)methyl]pyrrolo[1,2,3-de]-1,4-benzoxazin-yl]-(1-naphthalenyl)methanone mesylate (R(+)-WIN 55212-2 mesylate) andS(−)-WIN 55212-3 mesylate were purchased from Research Biochemicals (Natick, MA) andN-(piperidin-1-yl)-5-(4-chlorophenyl)-1-(2,4-dichlorophenyl)-4-methyl-1H-pyrazole-3-carboxamidehydrochloride (SR141716A) was obtained from the National Institute on Drug Abuse. Drugs were dissolved in dimethylsulfoxide (DMSO) and given as 300 μl injections by the intraperitoneal route, 40 min before occlusion of the CCAs (global ischemia) or 30 min before or 30, 60, or 120 min after MCA occlusion (focal ischemia). R(+)-WIN 55212-2 produced dose-dependent behavioral effects consisting of slight drowsiness (1 mg/kg), more marked drowsiness with limb rigidity and hypokinesia in ∼50% of animals (3 mg/kg), and more severe rigidity and hypokinesia in 100% of animals (10 mg/kg).

Quantification of neuronal loss. Three days after exposure to global ischemia, animals were perfused transcardially with 200 ml of saline and then 300 ml of 4% paraformaldehyde in 0.1 Mphosphate buffer, pH 7.4, and killed by decapitation. The brains were removed and post-fixed in the same paraformaldehyde solution for 5 d and then embedded in paraffin, and 6 μm sections through the dorsal hippocampus (anteroposterior coordinate, bregma − 3.0 mm) were cut on a microtome and processed for staining with cresyl violet. Neuronal counts in a predesignated region of CA1 were obtained from six to eight animals per condition.

Quantification of infarct volume. Rats subjected to focal ischemia were anesthetized with an overdose of chloral hydrate and decapitated. The brains were removed and sectioned coronally at 2 mm intervals. Sections were immersed in 2% 2,3,5-triphenyltetrazolium hydrochloride (TTC) in saline for 20 min at 37°C and then fixed for 30 min in 4% paraformaldehyde (Isayama et al., 1991). Six sections per brain were analyzed for infarct size using a computerized image analysis system (MCID, St. Catharine's, Ontario, Canada). Infarct area in each section was calculated by subtracting the residual uninfarcted, TTC-stained area of the ischemic (left) hemisphere from the total area of the nonischemic (right) hemisphere (Swanson et al., 1990). Infarct volume at 24 hr measured in this manner is equivalent to infarct volume determined from hematoxylin- and eosin-stained sections (Isayama et al., 1991).

Neuronal cell culture. Neuronal cultures were prepared from 16—17 d Sprague Dawley rat embryos (Yu et al., 1986). Cerebral hemispheres were removed aseptically, freed of meninges, olfactory bulbs, basal ganglia, and hippocampi, and incubated at 37°C in Ca2+- and Mg2+-free Earle's balanced salt solution containing 0.01% trypsin (1:250). After 30 min, 10% horse serum (HS) was added. Cells were placed in 2 ml of fresh MEM, triturated, and resuspended in Eagle's MEM prepared without glutamine and with twice the usual concentration of other amino acids and four times the usual concentration of vitamins (MEM-Pak; Cell Culture Facility, University of California, San Francisco, CA); this medium had been supplemented on the day of plating with glucose (final concentration, 30 mM), 2 mM glutamine, and 15 mM HEPES, pH 7.4. Cell suspensions were filtered through a 70 μm Falcon nylon cell strainer, supplemented with 10% HS and 10% fetal bovine serum (FBS), and seeded at 3 × 105 cells per well on 24-well Corning (Corning, NY) tissue culture dishes coated with 100 μg/ml poly-D-lysine. Cultures were incubated for 20 min at 37°C in humidified 95% air and 5% CO2, and one-half of the medium was replaced with medium containing 5% HS and 5% FBS. Cytosine arabinoside (AraC, 10 μM) was added on the sixth day in vitro (DIV). At 7 DIV, two-thirds of the medium was replaced with medium lacking AraC; thereafter, one-half of the medium was replaced with fresh medium twice weekly. Experiments were conducted at 18 DIV, when cultures consisted primarily of neurons (92 ± 1% MAP2-immunoreactive cells, 6 ± 1% GFAP-immunoreactive cells;n = 12).

In vitro model of ischemia. To model neuronal ischemia in vitro, cultures were exposed to combined hypoxia and glucose deprivation (Koretz et al., 1994). Two-thirds of the medium was replaced three times with serum-free medium, with or without 30 mM glucose. Glucose-containing cultures were then incubated for 24 hr at 37°C in humidified 95% air and 5% CO2. Glucose-deprived cultures were placed in a Billups-Rothenberg (Del Mar, CA) modular incubator chamber, which was flushed for 5 min with 95% N2 and 5% CO2, sealed for 15 min, flushed again for 30 sec with 5% N2 and 5% CO2, and resealed. The chamber was placed in a water-jacketed incubator at 37°C for 8 hr and then returned to 95% air and 5% CO2 and glucose-containing medium for 16 hr. In some experiments, glucose-containing, normoxic cultures were treated for 8 hr with and then 16 hr without 1 mM NMDA or 1 mM AMPA in the presence or absence of the NMDA antagonist (5R,10S)-(+)-5-methyl-10,11-dihydro-5H-benzo[a,d]cyclohepten-5,10-imine hydrogen maleate (MK-801) or the AMPA antagonist 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) (all from Research Biochemicals, Natick, MA). Stock solutions of cannabinoid receptor agonists and antagonists were prepared in DMSO and diluted to a final concentration not exceeding 7.36 μM DMSO in the drug-treated cultures. At concentrations at least 10-fold higher than this, DMSO had no effect on neuronal viability in either normoxic or hypoxic cultures.

Cytotoxicity assays. Fluorescence of Alamar blue (Accumed International, Westlake, OH), an indicator that changes color from blue to red and fluoresces when reduced by cellular metabolic activity, was used to measure the viability of cultured neurons. One-half of the culture medium was replaced with MEM-Pak containing 10% (v/v) Alamar blue, and cultures were incubated for 3 hr at 37°C in humidified 95% air and 5% CO2. Fluorescence was determined in a Millipore (Bedford, MA) CytoFluor 2300 automated plate-reading fluorometer, with excitation at 530 nm and emission at 590 nm. As reported previously, Alamar blue fluorescence in these cultures varies linearly with cell number, decreases with exposure to hypoxia or excitotoxins, and correlates with the extent of cellular injury determined by lactate dehydrogenase release (White et al., 1996).

Detection of DNA damage. DNA polymerase I-mediated biotin-dATP nick translation (PANT) labeling was used to detect DNA single-strand breaks (Didier et al., 1996). Cultures were fixed for 15 min at room temperature by adding 20% paraformaldehyde in PBS, pH 7.4, to a final concentration of 4%, washed three times with PBS, and permeabilized for 10 min with 0.5% Triton X-100 in PBS. H2O2 (1%) was added for 15 min at room temperature to neutralize endogenous peroxidase, after which cultures were again washed three times with PBS. Cells were then incubated for 60 min at 37°C in PBS, pH 7.6, containing 5 mMMgCl2, 10 mM 2-mercaptoethanol, 50 μg/ml bovine serum albumin (BSA), 20 μM dCTP, dGTP, dTTP, and biotinylated-dATP, and 50 U/ml Escherichia coliDNA polymerase I (Sigma, St. Louis, MO). Cells were washed three times with ice-cold PBS and once with 5 mg/ml BSA in PBS (PBS-BSA), incubated for 1 hr at room temperature with streptavidin-horseradish peroxidase (HRP) in PBS-BSA (Vector Laboratories, Burlingame, CA), and washed four times in PBS. The HRP complex was detected after incubation for 5 min at room temperature in PBS containing 0.5 mg/ml diaminobenzidine, 0.03% H2O2, and nickel (added according to the manufacturer's instructions). Cells with dense nuclear staining were considered PANT-positive and were counted at 200× magnification in at least three randomly selected fields per well. Data were expressed as a percentage of all cells in the same fields, with reactions conducted in the absence of DNA polymerase I serving as controls for nonspecific labeling.

Statistical analysis. Results are reported as mean values ± SE. The significance of differences between means was assessed by Student's t test (single comparisons) or by ANOVA and post hoc t tests (multiple comparisons), with p < 0.05 considered statistically significant.

RESULTS

Global cerebral ischemia
In control animals that underwent sham CCA occlusions, ∼300 neurons could be counted in the designated region of CA1, whereas only zero to five neurons were seen after global ischemia (Figs.1, 2).R(+)-WIN 55212-2, a synthetic aminoalkylindole cannabimimetic compound, competes with THC for binding to cannabinoid receptor sites in brain (Kuster et al., 1993) and reproduces pharmacological and behavioral effects of THC (Compton et al., 1992). When animals were given R(+)-WIN 55212-2 mesylate intraperitoneally 40 min before the induction of global cerebral ischemia, there was a dose-dependent increase in neuronal survival that reached maximal levels (56% of sham-operated controls) at 1 mg/kg. At higher doses, neuronal survival declined. The doses that protected against ischemic neuronal death were similar to those associated with behavioral actions such as locomotor inhibition, antinociception, and THC-like discriminative effects (Compton et al., 1992). Neuroprotection by R(+)-WIN 55212-2 (1 mg/kg) was not associated with significant changes before, during, or after the induction of ischemia in mean arterial blood pressure, PaO2, PaCO2, pH, or blood glucose concentration compared with values in animals that received DMSO vehicle alone (Table1).

R(+)-WIN 55212-2 is one of a pair of enantiomers that exhibit stereoselectivity in cannabinoid receptor radioligand binding assays and behavioral studies. R(+)-WIN 55212-2 has ∼2500-fold greater affinity than its enantiomer, S(−)-WIN 55212-3, for CB1 receptor binding sites on rat cerebellar membranes (Kuster et al., 1993), and the S(−) enantiomer is inactive in behavioral assays of cannabimimetic activity that show potent effects of R(+)-WIN 55212-2 (Compton et al., 1992). When animals were treated with S(−)-WIN 55212-3 before ischemia, neuronal counts in CA1 were not significantly different from counts obtained after ischemia alone and were significantly lower than counts in animals given R(+)-WIN 55212-2.

SR141716A is a selective, competitive antagonist that inhibits radioligand binding to CB1 cannabinoid receptors in rat brain synaptosomal membranes, cannabinoid-induced inhibition of smooth muscle contraction in mouse vas deferens, and behavioral effects ofR(+)-WIN 55212-2, including locomotor inhibition and antinociception (Rinaldi-Carmona et al., 1994). When administered alone before ischemia, SR141716A failed to alter neuronal counts. However, when 1 mg/kg SR141716A was given together with 1 mg/kgR(+)-WIN 55212-2, the neuroprotective effect of the latter was reduced by 80%.

Focal cerebral ischemia
MCA occlusion produced ipsilateral cerebral infarcts averaging ∼210 mm3 in volume, which could be detected after 24 hr by the loss of TTC staining (Figs.3, 4). Pretreatment with 1 mg/kg R(+)-WIN 55212-2 given 30 min before the onset of ischemia reduced infarct size by ∼30%. The drug was similarly effective when given 30 min after the onset of ischemia, but its effect was lost when administration was delayed by 60—120 min. Cerebral salvage occurred primarily in the periphery of the ischemic region, leading to enhanced survival of penumbral cortical tissue, without affecting the ischemic core in the striatum. Reduction of infarct size by R(+)-WIN 55212-2 (1 mg/kg) was not accompanied by alterations in mean arterial blood pressure, PaO2, PaCO2, pH, or blood glucose concentration, measured 10 min after the onset of ischemia, compared with values in control animals given DMSO vehicle alone (Table 2).

The CB1 cannabinoid receptor antagonist SR141716A had no effect on infarct size when administered alone but reversed the protective effect of R(+)-WIN 55212-2 given 30 min before the onset of ischemia. The less active agonist isomer,S(−)-WIN 55212-3, failed to alter infarct volume.

In vitro hypoxia and glucose deprivation
Both normoxic and hypoxic cortical cultures expressed CB1 receptor immunoreactivity on Western blots probed with a polyclonal rabbit IgG (Calbiochem, La Jolla, CA) raised against the N-terminal domain of the human CB1 receptor (Fig.5 A). Exposure of cortical cultures to hypoxia and glucose deprivation reduced neuronal viability (Alamar blue fluorescence), with approximately half-maximal toxicity at 8 hr and maximal toxicity by 24 hr. The NMDA antagonist MK-801 reduced toxicity, as did R(+)-WIN 55212-2 and the endogenous cannabinoid anandamide (Fig. 5 B). Exposure for 8 hr to 1 mM NMDA or AMPA decreased neuronal viability to an extent similar to that seen with hypoxia and glucose deprivation, but although MK-801 blocked NMDA toxicity, and the AMPA antagonist CNQX blocked AMPA toxicity under these conditions, R(+)-WIN 55212-2 was ineffective (data not shown). PANT staining, indicative of cells with DNA single-strand breaks (Chen et al., 1997), also increased after hypoxia and glucose deprivation, and this increase was attenuated by both MK-801 and R(+)-WIN 55212-2 (Fig.6).

To test whether the same CB1 receptor-mediated mechanism involved in protection from in vivo ischemia was also responsible for in vitro neuroprotection byR(+)-WIN 55212-2, we examined the effects of the less-active enantiomer S(−)-WIN 55212-3, the CB1 agonists anandamide and THC, the CB1 antagonist SR141716A, and the CB2 antagonistN-[(1S)-endo-1,3,3-trimethyl bicyclo[2.2.1]heptan-2-yl]-5-(4-chloro-3-methylphenyl)-1-(4-methylbenzyl)-pyrazole-3-carboxamide (SR144528; obtained from the National Institute on Drug Abuse) (Rinaldi-Carmona et al., 1998). As shown in Figure 5 B, protection from hypoxia and glucose deprivation in our cultures did not have the pharmacological features of a CB1 or CB2 receptor-mediated process. Thus, although the endogenous cannabinoid anandamide reduced hypoxic injury, THC did not. Moreover, neuroprotection lacked stereoselectivity and was insensitive to CB1 and CB2 antagonists. As was also observed in our studies on global ischemia, the protective effect ofR(+)-WIN 55212-2 was lost at higher concentrations (Fig.5 C).

DISCUSSION

The major finding we report is that the synthetic cannabinoidR(+)-WIN 55212-2, an analog of the psychoactive constituents of marijuana, protects brain tissue against ischemic injury. This effect appears to be mediated through CB1 cannabinoid receptors, because it is stereospecific and is blocked by a selective CB1 receptor antagonist, SR141716A. We observed neuroprotection by R(+)-WIN 55212-2 in both global and focal ischemia and, in the latter case, with drug administration either before or up to 30 min after the onset of ischemia. Cannabinoid-mediated protection from global ischemia was seen in the CA1 region of hippocampus, which is especially vulnerable to ischemic injury, and inhibition of glutamate release by cannabinoids has been demonstrated in cells cultured from this region (Shen et al., 1996). Cannabinoid receptor levels in hippocampus, including CA1, and in cerebral cortex, which was the major site of cannabinoid-mediated neuroprotection in our focal ischemia model, are among the highest in the brain (Matsuda et al., 1990; Kuster et al., 1993; Adams et al., 1998).

In principle, the neuroprotective action of R(+)-WIN 55212-2 could be exerted in a variety of ways. For example, the ability of cannabinoids to inhibit ion flux through calcium channels (Mackie and Hille, 1992) and thereby reduce glutamate release (Shen et al., 1996) suggests that these effects could be responsible for neuroprotection. However, cannabinoid receptor activation has been shown to affect a variety of second mesenger systems, including the cAMP and phospholipase A2—cyclooxygenase signal transduction pathways (Chan et al., 1998), so reduction of calcium influx may not necessarily be responsible for cannabinoid-mediated neuroprotection. The vasoactive properties of cannabinoids (Randall and Kendall, 1998) raise the possibility that they may alter blood flow in the ischemic brain, but although it would be premature to conclude that such alterations have no role in the neuroprotective effect of cannabinoids, a major contribution of altered blood flow seems unlikely. Protection was seen not only in focal ischemia, in which blood flow might be redistributed from nonischemic to ischemic brain regions, but also in global cerebral ischemia, which affects the brain diffusely. Moreover, isoelectricity of the electroencephalogram, reflecting ischemia severe enough to interrupt brain function, was present during global ischemia in both cannabinoid-treated and untreated animals, arguing against cannabinoid-induced preservation of cerebral blood flow. Cannabinoids can also promote hypothermia, which is neuroprotective in some settings. Although rectal and brain temperature were held constant during the early stages of our global and focal ischemia studies, a contributory effect of late hypothermia on outcome cannot be excluded. Finally, cannabinoids exert anti-inflammatory effects, at least in part by inhibiting the proliferation of lymphocytes and inducing their death by apoptosis (Schwarz et al., 1994), and inflammation has been implicated in focal ischemic brain injury (Nogawa et al., 1997). However, inflammation appears to be a less prominent feature of transient global cerebral ischemia (Dirnagl et al., 1994), in which we found neuroprotection by cannabinoids similarly effective.

We also observed neuronal protection in an in vitro cell culture model of neuronal hypoxia and glucose deprivation, but the mechanism appeared to differ from that observed in vivo. In particular, neuroprotection in vitro lacked stereoselectivity for R(+)-WIN 55212-2 overS(−)-WIN 55212-3 and was insensitive to inhibition by cannabinoid receptor antagonists. This resembles in some respects the effect reported by Hampson et al. (1998b), who found that comparatively high concentrations of THC reduced excitotoxicity in cultured cortical neurons by a receptor-independent mechanism. In contrast to those investigators, however, we found no effect of THC and no protection against directly applied excitatory amino acids or the nitric oxide donor sodium nitroprusside (data not shown), arguing against an antioxidant effect such as that they proposed. Whether the nonreceptor-mediated neuroprotective effect of cannabinoids that we observed in vitro also operates in vivo is unclear, although there is precedent for the coexistence of parallel, receptor-mediated and non-receptor-mediated effects of cannabinoids on neurotransmission and signal transduction (Felder et al., 1992; Hampson et al., 1998a). Therefore, it would not be altogether surprising if similarly parallel neuroprotective mechanisms were found.

Two other in vitro studies of cannabinoid effects have appeared recently and require comment. One described a toxiceffect of THC on cultured hippocampal neurons (Chan et al., 1998), and the other showed a protective effect of R(+)-WIN 55212-2 on cultured hippocampal neurons exposed to excitotoxicity induced by Mg2+ depletion (Shen and Thayer, 1998). Both effects appeared to be CB1 receptor-mediated. Thus, neurotoxic and neuroprotective–as well as receptor-mediated and non-receptor-mediated–effects of cannabinoids can be observed in vitro. These differences are likely to depend on a variety of influences, apparently including the nature of the toxic insult, the source of cells, and the particular cannabinoid used. In light of our finding that cannabinoids afford receptor-mediated neuroprotection against global and focal cerebral ischemia in vivo(occurring in hippocampus and cerebral cortex, respectively), the discrepant results of our and other in vitro studies accent the importance of using in vivo models to establish how potential therapeutic agents are likely to affect intact organisms.

Whether the in vivo protective effect of cannabinoids that we observed is permanent or only delays ischemic death beyond the time frames examined remains to be shown, as does the relationship between histological and functional improvement. Nevertheless, the ability of cannabinoids to improve histological outcome after both global and focal cerebral ischemia in rats indicates that further investigation of its potential therapeutic role in cerebral ischemia, such as occurs in stroke and after cardiac arrest, may be warranted.

Source, Graphs and Figures: Cannabinoids and Neuroprotection in Global and Focal Cerebral Ischemia and in Neuronal Cultures
 
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