In contrast to the numerous reports on the pharmacological effects of Δ⁹-tetrahydrocannabinol (THC), the pharmacological activity of another substituent of Cannabis sativa, cannabichromene (CBC) remains comparatively unknown. In the present study, we investigated whether CBC elicits cannabinoid activity in the tetrad assay, which consists of the following four endpoints: hypomotility, antinociception, catalepsy, and hypothermia. Because cannabinoids are well documented to possess anti-inflammatory properties, we examined CBC, THC, and combination of both phytocannabinoids in the lipopolysaccharide (LPS) paw edema assay. CBC elicited activity in the tetrad that was not blocked by the CB₁ receptor antagonist, rimonabant. Moreover, a behaviorally inactive dose of THC augmented the effects of CBC in the tetrad that was associated with an increase in THC brain concentrations. Both CBC and THC elicited dose-dependent anti-inflammatory effects in the LPS-induced paw edema model. The CB₂ receptor, SR144528 blocked the anti-edematous actions of THC, but not those produced by CBC. Isobolographic analysis revealed that the anti-edematous effects of these cannabinoids in combination were additive. Although CBC produced pharmacological effects, unlike THC, its underlying mechanism of action did not involve CB₁ or CB₂ receptors. In addition, there was evidence of a possible pharmacokinetic component in which CBC dose-dependently increased THC brain levels following an i.v. injection of 0.3 mg/kg THC. In conclusion, CBC produced a subset of behavioral activity in the tetrad assay and reduced LPS-induced paw edema through a noncannabinoid receptor mechanism of action. These effects were augmented when CBC and THC were co-administered.

2.1. Animals

Studies utilized male ICR mice (Harlan Laboratories, Dublin, VA) weighing 20 – 30 g that were housed six to a cage in the animal care facility maintained at 22 ± 2°C on a 12 h light/dark cycle. Food and water were available ad libitum and mice were given 24 h to acclimate to the test environment (22 ± 2°C) before analysis; animals were housed in the test environment until the termination of experimental procedures for LPS-induced inflammation studies. All animal studies were approved by the Institutional Animal Care and Use Committee of Virginia Commonwealth University in accordance with the National Institute of Health Guide for the Care and Use of Laboratory Animals.

2.2. Drugs

CBC was synthesized from Organix Inc. (Woburn, MA), and THC, rimonabant, and SR144528 were supplied by the National Institute on Drug Abuse (Bethesda, MD). All compounds were dissolved in a vehicle consisting of absolute ethanol, alkamuls-620 (Rhone-Poulenc, Princeton, NJ), and saline in a ratio of 1:1:18. For tetrad experiments, all injections were administered intravenously in a volume of 0.1 ml per 10 g of body weight. For LPS-induced inflammation studies, drugs were administered intraperitoneally in a volume of 0.1 ml per 10 g of body weight. LPS from Escherichia coli 026:B6 (Sigma-Alrich, St. Louis) was suspended in 0.9% saline for paw administration.

2.3. Tetrad procedure

Pretreatment baseline tail-flick response to radiant heat (D’Amour et al., 1941) and rectal temperature were recorded. The intensity of the radiant heat stimulus was held constant to yield control latencies of 2 – 4 seconds with an automated cut-off of 10 s to prevent tissue damage to the tail. Rectal temperatures were taken with a digital thermometer (Fisher Scientific, Pittsburgh, PA) at a depth of 2 cm and recorded to the nearest 0.1°C. Locomotor suppression, antinociception, hypothermia, and catalepsy were evaluated (in that respective order) after the mice received drug treatment. Five min post-drug administration, mice were placed in individual activity chambers (plastic mouse cages in a dark cabinet) surrounded by photocell beams (Digiscan Animal Activity Monitor; Omnitech Electronics, Inc., Columbus, OH). Locomotor suppression was measured for 10 min and the data were expressed as the total number of photocell beam breaks. Tail-flick latency was measured at 20 min after drug administration. Antinociception was calculated as a percent of maximum possible effect (%MPE) by the following formula: %MPE = [(test latency-pretreatment latency)/(10-pretreatment latency)] × 100}. At 30 min, rectal temperature was measured and data were expressed as the difference between pretreatment rectal temperature and post-injection rectal temperature. At 40 min, mice were evaluated for catalepsy in a 5 min ring immobility test (Gill et al., 1970; Pertwee, 1972) in which each subject was placed on a metal ring (5.5 cm diameter) that was suspended 16 cm from the benchtop with a black background board attached (for contrast with the albino mice). The total duration of time spent motionless (no voluntary movement) was timed using a stopwatch.

2.4. Extraction Procedure, GC/MS Analysis

Mice were decapitated at two different time points (discussed in results section) and the blood was collected in heparinized tubes (Fisher Scientific, Pennsylvania). Whole brains were harvested and stored on ice until homogenized. Brain tissue was homogenized less than two h following the harvest in a 2:1 ratio (vol/wt) of saline to brain tissue. Aliquots (0.5 ml) were prepared from heparinized mouse whole blood or homogenized brain tissue. Calibrators were prepared by adding drug standards to naïve mouse blood and brain tissue. Fifty µl of internal standard (THC-d₃; Cerilliant, Round Rock, Texas) was added to all calibrators and samples (minus blank samples). All tubes were equilibrated overnight at 5°C.

“Ice cold” acetonitrile (2 ml) was added dropwise while vortexing and the mixture was centrifuged at 3,000 rpm for 10 minutes. The mixture was stored overnight at −30°C to assist in further separation of the layers. The top layer (acetonitrile layer) was isolated and 2 ml of 0.2 N NaOH was added while vortexing the tubes. Four ml of organic solvent (9:1, hexane:ethyl acetate) was added and the tubes were rotated at 30 rpm for 30 min. The tubes were then centrifuged at 3,000 rpm for 10 min. The organic layer was isolated and evaporated to dryness in a Savant AES1000. Fifty µl of derivatizing agent (RC3; Regis Technologies, Inc., Morton Grove, IL) was added to each tube and samples were heated at 70°C for 20 min. Samples were then transferred to microvials for GC/MS analysis.

Microvials were loaded on a Shimadzu QP2010 GC/MS utilizing a splitless injection port and DB-5 column (30 m × 0.25 mm I.D. × 25 µm film thickness). The GC/MS was operated under the following temperatures: initial, 190°C; ramp, 30°C/min to 330°C then hold 1 min; injection port, 250°C; transfer line, 280°C; and ion source, 260°C. Ions monitored in SIM mode: 315, 343, 386 m/z for THC; 303, 246, 371 m/z for CBC; and 346, 389 m/z for THC-d₃. Calibration curves were constructed with at least six calibrators to extend the linearity range for appropriate experiments.

2.5. Inflammation Induction and Measurement Procedure

Baseline body weights, as well as paw thicknesses of both hind paws were measured two h before LPS injection and again 24 h later. Digital calipers (Fisher Scientific, Inc., Pittsburgh, PA) were utilized to measure paw thickness to the nearest 0.01 mm. In accordance with a previously described method (Naidu et al., under review), mice received a subcutaneous injection (utilizing a 30 gauge needle) of LPS (25 µg in 50 µl of saline) into the plantar region of a hind paw. As a control, the contralateral hind paw received a 50 µl injection of saline in the same manner as previously stated. Paw thickness data are depicted as the change in paw thickness from baseline for the LPS-injected (ipsilateral) or saline-injected (contralateral) hind paws.

Mice received intraperitoneal injections of test drugs 1 h before, as well as 6 and 23 h after LPS injection. In experiments evaluating cannabinoid receptor mechanisms of action, rimonabant, SR144528, or vehicle was administered 30 min prior to each injection of vehicle, THC, or CBC at the three respective drug administration time points. In the drug interaction study, CBC and THC doses were combined and administered as a single injection at the three respective time points.

2.6. Statistical Analyses

Behavioral data and concentrations of cannabinoids in blood and brain matrices were statistically analyzed using ANOVA in Statview 5.0 (SAS Institute Inc., Cary, N.C.) or Prism 5 (Graphpad Software, Inc., San Diego, CA). When ANOVA yielded significant results, Dunnett’s test (comparison of all treatment groups to a vehicle group in dose-response studies) or Tukey’s test (comparison of all groups) was used for post hoc analysis. Bonferonni’s t-test was used for planned comparisons. A p value of less than 0.05 was denoted as significant for all analyses. Linear regression analysis of calibration curves and cannabinoid concentrations in blood and brain tissue were determined in Prism 5. For all experiments, unless otherwise indicated, n=6 mice per group.

Isobologram analysis (Tallarida et al., 1989; Tallarida, 2001;Tallarida, 2006) was used to determine the nature of the interaction between co-administration of THC and CBC in the above assays. Experimental ED₅₀ values from combination doses that are along the line of additivity confer an additive relationship, below the line a synergistic relationship, and above the line an antagonistic relationship. A theoretical additive ED₅₀ value of both drugs in combination (calculated from the ED₅₀ value of each drug’s separate dose-response curve) was compared to the experimental ED₅₀ value of both drugs in combination. A 1:1 ratio of three combination drug doses (calculated from each drug’s ED₅₀ value and two descending log doses) was utilized in the experiment to determine the experimental ED₅₀. The experimental ED₅₀ (with confidence intervals) was then graphically compared to the theoretical additive ED₅₀ value (with confidence intervals) to determine if these values overlapped (indicative of an additive relationship between the two drugs). Prism 5 and PharmTools Pro 1.1 (PharmSoft, Wynnewood, PA) were utilized for isobologram analysis.

3.1. CBC elicits pharmacological effects through a non-CB₁receptor mechanism of action in the tetrad assay

The effects of intravenously administered CBC (3, 10, 30, or 100 mg/kg) in the tetrad assay are shown in Figure 1. CBC caused significant locomotor suppression (Panel A; F[4,25]=7.9, p<0.001), catalepsy (Panel B; F[4,25]=6.7, p<0.001), antinociception (Panel C; F[4,25]=3.6, p<0.05), and hypothermia (Panel D; F[4,25]=14.0, p<0.001). However, only the largest dose of CBC tested (i.e., 100 mg/kg) produced significant effects in each of these measures (Dunnett’s post hoc, p<0.05). The effects of the high dose of CBC (100 mg/kg) in the tetrad assay were then compared to those produced by THC. Significant effects of treatment for locomotor suppression (Supplementary Figure 1A1; F[5,30]=14.1, p<0.001), catalepsy (Figure 1B1; F[5,30]=36.1, p<0.001), antinociception (Figure 1C1; F[5,30]=38.0, p<0.001), and hypothermia (Figure 1D1; F[5,30]=59.2, p<0.001) were found. Dunnett’s post hoc analysis (p<0.05) revealed that THC (3 and 10 mg/kg) and CBC (100 mg/kg) produced significant locomotor suppression, catalepsy, and hypothermia compared to vehicle control mice. However, in this experiment, CBC did not elevate tail-flick latencies, though THC (1, 3, and 10 mg/kg) produced significant antinociception.

Figure 1

Comparison between the dose-response of intravenously administered CBC alone and in combination with an inactive dose of THC (i.e., 0.3 mg/kg) in the mouse tetrad. When given alone, only 100 mg/kg CBC produced locomotor suppression (A), catalepsy (B), …

In the next experiment, we investigated whether CB₁ receptors mediate the effects of CBC in the tetrad assay. Mice were given an injection of vehicle or rimonabant (3 mg/kg) followed 10 min later by a second injection of vehicle or CBC (100 mg/kg). This dose of the CB₁ receptor antagonist is sufficient to block the pharmacological effects of THC and other cannabinoid receptor agonists in the tetrad assay (Compton et al., 1996). As can be seen in Figure 2, CBC produced significant hypomotility (Panel A; F[1,19]=9.7, p<0.01), catalepsy (Panel B; F[1,19]=21.5, p<0.001), and hypothermia (Panel D;1 ²F[1,19]=11.5, p<0.01), but not antinociception (Panel C; p=0.09). In contrast, there were no significant main effects of rimonabant or interactions between CBC and rimonabant for any of the four dependent ³ measures, indicating that CBC produces these pharmacological effects through a non CB₁ receptor mechanism of action.

Figure 2

The pharmacological effects of CBC for locomotor suppression (A), catalepsy (B), antinociception (C), and hypothermia (D) are not mediated by the CB₁ receptor. Mice were intravenously administered an i.p. injection of vehicle or rimonabant (3 mg/kg) followed …

3.2. THC enhances the pharmacological effects of CBC

In the next experiment, we sought to determine whether a threshold dose of THC could augment the pharmacological effects of CBC in the tetrad assay. Based on the THC dose-response curves (Supplementary Figure 1), 0.3 mg/kg THC was selected as the threshold dose. Subjects received an i.v. injection of vehicle or CBC (3, 10, 30, or 100 mg/kg) 10 min before an i.v. injection of 0.3 mg/kg THC. As can be seen in Figure 1, 0.3 mg/kg THC produced a leftward shift in the CBC dose-response curves of CBC for catalepsy, antinociception, and hypothermia, but not hypomotility. Significant effects were found for locomotor activity (Figure 1A; F[5,30]=3.5, p<0.05), catalepsy (Figure 1B; F[5,30]=34.4, p<0.0001), antinociception (Figure 1C; F[5,30]=8.2, p<0.0001), and hypothermia (Figure 1D; F[5,30]=13.8, p<0.0001).

Because a threshold dose of THC significantly enhanced most of the pharmacological effects of CBC, the concentrations of both phytocannabinoids in blood and brain tissue were quantified to determine whether the drugs given in combination may have altered the pharmacokinetics of each other. Mice received an injection of CBC (vehicle, 3, 10, 30, or 100 mg/kg) followed 10 min later with a second injection of THC (0.3 mg/kg) or no injection. Tissues were harvested 30 min after CBC. Although CBC did not significantly affect THC blood levels (Figure 3A; p=0.07), it led to a dose-related increase in THC brain levels (Figure 3B; F[4,24]=9.9, p<0.001). Not surprisingly, increasing doses of CBC led to significant increases of this compound in blood (F[7,39]=12.6, p<0.001; Figure 3C) and brain (F[7,40]=67.0, p<0.0001; Figure 3D), but there were no effects of THC on CBC blood and brain levels. These results indicate that CBC dose-dependently elevated THC brain levels, but the threshold dose of THC did not affect CBC brain or blood levels.

Figure 3

Quantification of blood and brain tissue concentrations of THC and CBC in mice administered a dose range of CBC with and without an inactive dose of THC. Mice were given an i.v. injection of CBC (vehicle, 3, 10, 30, or 100 mg/kg) followed by a second …

3.3. Evaluation of CBC and THC on LPS-induced paw edema

Both CBC (F[4,25]=8.3, p<0.001) and THC (F[4,25]=10.7, p<0.0001) produced dose-related decreases in LPS-induced paw edema (Figure 4A), but neither drug affected the paw thickness of the saline-injected paw (data not shown). Post hoc analyses indicated significant decreases in paw thickness of the LPS-injected paw following 10, 30, and 100 mg/kg CBC as well as 10 and 30 mg/kg THC compared to the respective vehicle control groups.

Figure 4

Distinct receptor mechanisms of action mediate the anti-edematous effects of THC and CBC. A. Anti-edematous effects of i.p. administered CBC and THC. Neither drug affected paw thickness in the contralateral paw (data not shown). The results are presented…

In order to determine whether CB₁ or CB₂ receptors mediated the anti-edematous effects of CBC and THC, mice were administered vehicle, rimonabant (3 mg/kg), or SR144528 (3 mg/kg) 30 min before each of the three injections of vehicle, CBC (100 mg/kg), or THC (10 mg/kg). A significant effect of treatment was found for the THC experiment (Figure 4B; F[5,30]=18.6, p<0.0001). Neither rimonabant nor SR144528 given alone affected LPS paw edema. SR144528, but not rimonabant, significantly reduced the anti-edematous effects of THC, indicating a CB₂ receptor mechanism of action.

As shown in Figure 4C, a significant effect of treatment was found in the CBC experiment (F[3,20]=7.3, p<0.01). However, neither rimonabant nor SR144528 ameliorated the anti-inflammatory effects of CBC, suggesting that the anti-edematous effects of this phytocannabinoid do not involve either CB₁ or CB₂ receptors.

3.4. Combination of CBC and THC on LPS-induced paw edema

In the final experiment, we examined whether equipotent doses of CBC and THC given in combination would to reduce LPS-induced paw edema in an additive or synergistic fashion. The dose-response relationship of the drugs given in 1:1 equipotent combination doses (4 mg/kg CBC:0.4 mg/kg THC, 12 mg/kg CBC:1.2 mg/kg THC, or 40 mg/kg CBC:4 mg/kg THC) are depicted in Figure 5. A significant effect of treatment (F[3,20]=5.4, p<0.0001) was found. Dunnett’s post hoc test revealed that the group treated with 40 mg/kg CBC:4 mg/kg THC had significantly less paw edema than the vehicle + vehicle control group (p<0.05). The ED₅₀ values (expressed as ED₅₀mg/kg (95% confidence intervals)) of CBC and THC calculated from their individual dose-response curves were 38.7 (23.9 to 62.5) and 4.0 (2.7 to 5.9) mg/kg, respectively. These ED₅₀ values were utilized to establish a line of additivity on the isobologram (Figure 5C). The experimental ED₅₀ value (95% confidence intervals) of CBC and THC in a 1:1 combination was 20.8 (11.1 to 38.7) mg/kg. The CBC and THC coordinates of the experimental ED₅₀ were calculated as 18.9 (10.1 to 35.2) and 1.9 (1.0 to 3.5) mg/kg, respectively. The theoretical ED₅₀ (located on the line of additivity was calculated as 21.3 (15.6 to 29.1) mg/kg and its CBC and THC coordinates were 19.3 (14.2 to 26.4) and 2.0 (1.5 to 2.7) mg/kg, respectively. Because the experimental and theoretical additive ED₅₀ values and confidences limits overlapped, the relationship between the two phytocannabinoids was additive.

Figure 5

The anti-inflammatory dose-response of CBC and THC administered in combination yield an additive interaction. Dose response curves from CBC alone (A) and THC alone (B) from Figure 4A. In the 1:1 combination study, mice were administered vehicle, 4 mg/kg …

4.1. Evaluation of pharmacological effects of CBC in the tetrad assay

CBC produced significant pharmacological effects only when administered at a high dose (i.e., 100 mg/kg), which consistently produced locomotor suppression, catalepsy, and hypothermia, but only occasionally produced a small magnitude of antinociception. The observation that CBC sporadically produced antinociception may indicate that there is a different threshold dose needed to produce this effect compared to the other three indices. Other cannabinoids have been shown to have different thresholds or potencies within each measure that make up the tetrad assay. For example, anandamide, which is an endogenous cannabinoid, had similar ED₅₀values for hypomotility, catalepsy, and hypothermia, but was 3 – 4 fold less potent in producing antinociception than the other measures after i.v. administration in wild type mice (Smith et al., 1994). In contrast, THC dose-dependently produced significant effects for each of the four measures, with high efficacy. These findings are consistent with previously reported tetrad effects of THC (Fan et al., 1994; Martin et al., 1991).

Considering the great disparity between mean percentages of THC (i.e., 8.8%) and CBC (i.e., 0.3%) from confiscated cannabis preparations seized in 2008 (Mehmedic, et al., 2010) as well as our observation that CBC is substantially less potent than THC in the tetrad, it is unlikely that CBC by itself relevantly contributes to the psychoactive effects of marijuana. This conclusion is in agreement with a previous study that reported the tetrad effects of marijuana were primarily accounted for by its THC content and not by the other constituents of this plant (Varvel et al., 2005). Another study that utilized human subjects varied the concentration of CBC in marijuana cigarettes and found that the CBC concentration in their cigarettes (0.01 – 2.31%) did not affect behavioral (cognitive tasks) or neurophysical measures (EEG, ERP) in the study (Ilan et al., 2005).

The CB₁ receptor antagonist, rimonabant failed to block the tetrad activity of CBC, indicating a non CB₁ receptor mechanism of action. These results are consistent with the observation that CBC possesses poor affinity to the CB₁ receptor (i.e., K_i value > 10,000 nM; Bookeret al., 2009). In comparison, rimonabant has been reported to have a K_i value of 2 nM and has been shown to block the tetrad effects of THC and other cannabinoids (Compton et al., 1996; Rinaldi-Carmona et al., 1994; Wiley et al., 1998). Various noncannabinoid classes of drugs have also been shown to have partial tetrad effects including central nervous system depressants and anti-psychotics that were not blocked by rimonabant (Wiley et al., 2003). Because the tetrad effects of CBC were not blocked by a CB₁ receptor antagonist, the mechanism by which CBC elicited tetrad effects remains to be established in future studies.

Another objective of the present study was to examine whether a threshold dose of THC would modify the pharmacological actions of CBC in the tetrad. An inactive dose of THC (i.e., 0.3 mg/kg) was selected based on a dose-response study of this compound in the tetrad assay. Administration of this dose of THC produced leftward shifts in the CBC dose-response relationship for catalepsy, antinociception, and hypothermia; however it did not enhance CBC-induced locomotor suppression. In order to test whether the enhanced pharmacological results occurred because of a pharmacokinetic interaction, we quantified blood and brain levels of CBC and THC given in combination. Although the behaviorally inactive dose of THC did not significantly alter CBC blood or brain concentrations, 30 or 100 mg/kg CBC led to significantly elevated THC levels in brain, but did not quite achieve statistical significance in affecting THC blood levels (p<0.07). These results suggest that THC had distributed out of the blood and into lipophilic matrices, such as brain, which is consistent with the reported pharmacokinetics of THC and its rapid distribution phase (Grotenhermen, 2003). About 90% of THC in blood is bound to plasma (10% to red blood cells) and 95 – 99% of plasma THC is bound to lipoproteins (Hunt et al., 1980; Widman et al., 1974). A high dose of CBC (30 or 100 mg/kg) may compete with THC (0.3 mg/kg) for the lipoprotein binding sites, which ultimately leads to the distribution of THC out of the blood and into lipophilic tissue such as the brain. Subsequently, the higher concentrations of THC in brain tissue might have interacted with CB₁ receptors to elicit significant tetrad activity. It is noteworthy that these same doses of CBC produced enhanced pharmacological effects when given in combination with the threshold dose of THC. Thus, it is plausible that a pharmacokinetic interaction between the two cannabinoids contributed to the leftward shift in the CBC dose response in the presence of 0.3 mg/kg THC. Taken together, these data suggest that high doses of CBC may augment a threshold dose of THC to produce significant cannabinoid activity in the tetrad.

4.2. Evaluation of CBC in the LPS-induced paw edema model

Recent research has demonstrated that WIN55,212-2, a potent mixed CB₁/CB₂ receptor agonist, URB597, a FAAH inhibitor, and dexamethasone, a synthetic glucocorticoid hormone ameliorated LPS induced paw edema (Naidu et al., under review). CBC as well as THC dose-dependently decreased LPS-induced inflammation in the LPS-injected paw. There are no prior reports in the literature that examined the anti-inflammatory effects of either of these cannabinoids in this inflammation model. The anti-edematous effects of THC were blocked by SR144528, but not by rimonabant, indicating that a CB₂ receptor mechanism of action. Other studies have also reported that the anti-inflammatory effects of THC are mediated though a CB₂ receptor mechanism (Croxford et al., 2005; Guzman et al., 2002; Klein, 2005). In marked contrast, the anti-inflammatory effects of CBC were not blocked by either SR144528 or rimonabant, indicating that its anti-inflammatory effects are mediated through a noncannabinoid receptor mechanism of action. Other phytocannabinoids have also been reported to have anti-inflammatory effects that are cannabinoid receptor independent. For example, the well documented anti-inflammatory effects of CBD are not blocked by cannabinoid receptor antagonists (Costa et al., 2004;Costa et al., 2007), though capsazepine, a TRPV1 receptor antagonist, has been found to block the anti-inflammatory actions of CBD in the carrageenan model. Furthermore, phytocannabinoids that exist as carboxylic acids have been reported to have anti-inflammatory effects that are not blocked by cannabinoid receptor antagonists. For example, a primary metabolite of THC, THC-COOH has been reported to have anti-inflammatory properties that may be mediated through suppression of cyclooxygenase and lipooxygenasein vitro (Burstein et al., 1986; Doyle et al., 1990) or through the activation of peroxisome-proliferative-activated receptor-γ (Liu et al., 2003). Because CBC is structurally related to these other phytocannabinoids, there may be a similar structure activity relationship in which the anti-inflammatory effects of CBC are mediated through receptors or processes similar to those underlying CBD or THC-COOH.

Isobolographic analysis was used to investigate anti-edematous interactions between CBC and THC. Examining the dose-response relationship of both compounds in which equipotent doses of the compounds were co-administered revealed an additive relationship. Accordingly, a benefit of this additive relationship is the possibility that these drugs administered in combination might produce anti-inflammatory effects at lower doses than each drug alone. Of course, it will be important to establish whether the psychotropic effects of THC are minimized, while still retaining anti-inflammatory efficacy.

4.3. Conclusions

In summary, CBC produced a subset of effects in the mouse tetrad assay and significantly reduced LPS-induced paw edema. Moreover, both of these effects were enhanced when CBC was given in combination with THC. The tetrad effects of CBC were not CB₁receptor mediated and its anti-inflammatory effects were not CB₁ or CB₂ receptor mediated. In contrast, we determined that THC produced its anti-inflammatory effects in the LPS-induced paw edema model via CB₂ receptor activation, a finding that had not been previously reported in this assay. Isobolographic analysis indicated an additive relationship between the anti-inflammatory effects of CBC and THC. A threshold dose of THC augmented the tetrad effects of CBC. However, the observation that high doses of CBC led to increased brain levels of THC suggests a potential pharmacokinetic interaction for the augmented tetrad effects of the two drugs given in combination.

In conclusion, CBC produced a subset of behavioral activity in the tetrad assay and reduced LPS-induced paw edema through a noncannabinoid receptor mechanism of action. Moreover, combination of CBC and THC leads to enhanced tetrad and anti-inflammatory actions.

01

Special thanks to Ramona Winckler for her help with intravenous injections and tetrad studies.

Role of Funding Source

This work was supported by the National Institute on Drug Abuse R01DA002396, R01DA03672, and R01 DA015683. NIDA had no further role in study design; in the collection, analysis and interpretation of the data; in the writing of the report; or in the decision to submit the paper for publication.

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^*A supplementary data figure is available with the online version of this article at doi:xxx/j.drugalcdep.xxx … Please see Appendix A.

¹See Appendix A.

Conflict of Interest

None of the authors report a conflict of interest that could have influenced, or be perceived to influence, this work.

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