USE OF CANNABIDIOL IN THE TREATMENT OF EPILEPSY

Abstract

The present invention relates to the use of cannabidiol (CBD) in the treatment of patients with childhood-onset epilepsy who are concurrently taking caffeine. Where the CBD is used in combination with caffeine, caution should be taken. For example, the dose of either the CBD and/or caffeine may be required to be reduced. Moreover, the patient may need to be monitored for side effects of said drug-drug interaction. Preferably the CBD used is in the form of a highly purified extract of cannabis such that the CBD is present at greater than 95% of the total extract (w/w) and the other components of the extract are characterised. In particular the cannabinoid tetrahydrocannabinol (THC) has been substantially removed, to a level of not more than 0.15% (w/w) and the propyl analogue of CBD, cannabidivarin, (CBDV) is present in amounts of up to 1%. Alternatively, the CBD may be a synthetically produced CBD.

Claims

1. Cannabidiol (CBD) for use in the treatment of childhood-onset epilepsy in patients who are concurrently taking caffeine characterised in that the blood levels of caffeine and associated markers are monitored to ensure the levels do not become toxic.

2. Cannabidiol (CBD) for use according to claim 1, wherein the dose of CBD is lowered.

3. Cannabidiol (CBD) for use according to claim 1, wherein the dose of caffeine is lowered.

4. Cannabidiol (CBD) for use according to claim 1, wherein the dose of CBD and caffeine is lowered.

5. Cannabidiol (CBD) for use according to any of the preceding claims, wherein blood levels of liver enzymes are monitored to ensure they do not become toxic.

6. Cannabidiol (CBD) for use according to any of the preceding claims, wherein the CBD is in the form of a highly purified extract of cannabis which comprises at least 95% (w/w) CBD.

7. Cannabidiol (CBD) for use according to claim 1, wherein the CBD is present as a synthetic compound.

8. Cannabidiol (CBD) for use according to claim 6, wherein the highly purified extract comprises less than 0.15% THC.

9. Cannabidiol (CBD) for use according to claim 6, wherein the extract further comprises up to 1% CBDV.

10. Cannabidiol (CBD) for use according to claim 2, wherein the lowered dose of CBD ranges from about 5 mg/kg/day to about 20 mg/kg/day.

11. Cannabidiol (CBD) for use according to claim 3, wherein the dose of caffeine is lowered to below 200 mg/day.

12. Cannabidiol (CBD) for use according to any of the preceding claims, wherein the childhood-onset epilepsy is: Lennox-Gastaut Syndrome; Myoclonic Absence Epilepsy; Tuberous Sclerosis Complex; Dravet Syndrome; Doose Syndrome; Jeavons Syndrome; CDKL5; Dup15q; Neuronal ceroid lipofuscinoses (NCL) and brain abnormalities.

13. A method of treating childhood-onset epilepsy in an individual in need thereof, comprising administering to the patient a therapeutically effective amount of cannabidiol with caution, wherein the individual is taking caffeine concurrently.

14. The method of claim 13, wherein said caution comprises lowering the dose of cannabidiol.

15. The method of claim 13, wherein said caution comprises lowering the dose of caffeine.

16. The method of claim 13, wherein said caution comprises monitoring said individual for side effects.

17. The method of claim 16, wherein said caution further comprises discontinuing cannabidiol if said side effects are observed.

18. The method of claim 13, wherein said caution comprises advising said individual of side effects from said concurrent therapy.

Description

BRIEF DESCRIPTION OF THE DRAWINGS

[0026] Embodiments of the invention are further described hereinafter with reference to the accompanying drawings, in which:

[0027] FIG. 1 shows Geometric Mean Plasma Concentrations of Caffeine Following Administration of Caffeine+Placebo (Day 1) and of Caffeine+CBD (Day 26) on a linear scale.

[0028] FIG. 2 shows Geometric Mean Plasma Concentrations of Paraxanthine Following Administration of Caffeine+Placebo (Day 1) and of Caffeine+CBD (Day 26) on a linear scale.

[0029] FIG. 3 shows Geometric Mean and Individual Subject C.sub.max for Caffeine and Paraxanthine Following Administration of Caffeine+Placebo (Day 1) and of Caffeine+CBD (Day 26).

[0030] FIG. 4 shows Geometric Mean and Individual Subject AUC0-∞ for Caffeine and Paraxanthine Following Administration of Caffeine+Placebo (Day 1) and of Caffeine+CBD (Day 26).

[0031] FIG. 5 shows Geometric LS Mean Ratio and 90% CI Showing the Effect of Steady-state CBD on Exposure to Caffeine and Paraxanthine.

[0032] FIG. 6 shows a Graph of serial liver chemistries for the 5 participants with ALT ULN.

DEFINITIONS

[0033] Definitions of some of the terms used to describe the invention are detailed below:

[0034] The cannabinoids described in the present application are listed below along with their standard abbreviations.

TABLE-US-00001 TABLE 1 Cannabinoids and their abbreviations CBD Cannabidiol [00001] CBDA Cannabidiolic acid [00002] CBDV Cannabidivarin [00003] CBDVA Cannabidivarinic acid [00004] THC Tetrahydrocannabinol [00005]

[0035] The table above is not exhaustive and merely details the cannabinoids which are identified in the present application for reference. So far over 60 different cannabinoids have been identified and these cannabinoids can be split into different groups as follows: Phytocannabinoids; Endocannabinoids and Synthetic cannabinoids (which may be novel cannabinoids or synthetically produced phytocannabinoids or endocannabinoids).

[0036] “Phytocannabinoids” are cannabinoids that originate from nature and can be found in the cannabis plant. The phytocannabinoids can be isolated from plants to produce a highly purified extract or can be reproduced synthetically.

[0037] “Highly purified cannabinoid extracts” are defined as cannabinoids that have been extracted from the cannabis plant and purified to the extent that other cannabinoids and non-cannabinoid components that are co-extracted with the cannabinoids have been substantially removed, such that the highly purified cannabinoid is greater than or equal to 95% (w/w) pure. The highly purified cannabinoid extract may be purified further such that the cannabinoid content is greater than or equal to 98% (w/w) pure.

[0038] “Synthetic cannabinoids” are compounds that have a cannabinoid or cannabinoid-like structure and are manufactured using chemical means rather than by the plant.

[0039] Phytocannabinoids can be obtained as either the neutral (decarboxylated form) or the carboxylic acid form depending on the method used to extract the cannabinoids. For example, it is known that heating the carboxylic acid form will cause most of the carboxylic acid form to decarboxylate into the neutral form.

[0040] “Childhood epilepsy” refers to the many different syndromes and genetic mutations that can occur to cause epilepsy in childhood. Examples of some of these are as follows: Dravet Syndrome; Myoclonic-Absence Epilepsy; Lennox-Gastaut syndrome; Generalized Epilepsy of unknown origin; CDKL5 mutation; Aicardi syndrome; tuberous sclerosis complex; bilateral polymicrogyria; Dup15q; SNAP25; and febrile infection related epilepsy syndrome (FIRES); benign rolandic epilepsy; juvenile myoclonic epilepsy; infantile spasm (West syndrome); and Landau-Kleffner syndrome. The list above is non-exhaustive as many different childhood epilepsies exist.

[0041] C.sub.max is the maximum observed plasma concentration.

[0042] t.sub.max is the time to attain maximum observed plasma concentration.

[0043] AUC.sub.0-∞ is the area under the plasma concentration-time curve from time 0 to infinity, calculated as AUC.sub.0-28=AUC.sub.0-t+Ĉ.sub.last/k.sub.el, where Ĉ.sub.last is the estimated last plasma concentration and where k.sub.el is the terminal phase rate constant.

[0044] AUC.sub.0-t is the area under the plasma concentration-time curve up to time t, where t is the last point with a concentration above the lower limit of quantification (LLOQ).

[0045] Clinical laboratory measurements of liver injury and function, the Upper Limit of Normal (ULN) values used are: 68 international units [IU]/L for ALT, 45 IU/L for aspartate aminotransferase (AST), 129 IU/L for alkaline phosphatase (ALP), 29 μmol/L for total bilirubin (TBL), and 59 IU/L for gamma-glutamyl transferase (GGT).

[0046] Drug induced liver injury (DILI) is when serum ALT exceeds 5×ULN.

DETAILED DESCRIPTION OF THE INVENTION

Preparation of Highly Purified Cbd Extract

[0047] The following describes the production of the highly-purified (>95-98% w/w) cannabidiol extract which has a known and constant composition was used in the Examples below.

[0048] In summary the drug substance used is a liquid carbon dioxide extract of high-CBD containing chemotypes of Cannabis sativa L. which had been further purified by a solvent crystallization method to yield CBD. The crystallisation process specifically removes other cannabinoids and plant components to yield greater than 98% CBD. Although the CBD is highly purified because it is produced from a cannabis plant rather than synthetically there is a small number of other cannabinoids which are co-produced and co-extracted with the CBD. Details of these cannabinoids and the quantities in which they are present in the medication are as described in Table 2 below.

TABLE-US-00002 TABLE 2 Composition of highly purified CBD extract Cannabinoid Concentration CBD >95-98% w/w CBDA NMT 0.15% w/w CBDV NMT 1.0% w/w Δ.sup.9 THC NMT 0.15% w/w CBD-C4 NMT 0.5% w/w >—greater than NMT—not more than

EXAMPLE 1: A PHASE 1, OPEN-LABEL, PHARMACOKINETIC DRUG-DRUG INTERACTION TRIAL TO INVESTIGATE THE EFFECT OF CANNABIDIOL ON THE PHARMACOKINETICS (PK) OF CAFFEINE

[0049] Primary Objectives: To investigate the effect of CBD treatment following repeated dosing on the PK of a single dose of caffeine in healthy subjects.

[0050] Primary Endpoints: The primary PK parameters were: AUC.sub.0-∞, AUC.sub.0-t, C.sub.max, and t.sub.max, for caffeine. The PK parameter endpoints, derived from the plasma concentration-time profiles of caffeine on Day 1 administered with placebo and the PK parameter endpoints derived from a single dose of caffeine in participants at steady state CBD following 13 days of CBD, 20 mg/kg twice daily (b.i.d).

[0051] Secondary Objectives: To evaluate the safety and tolerability of CBD when given with a single dose of caffeine in healthy subjects.

[0052] Secondary Endpoints: Safety includes: incidence and severity of adverse events (AEs), incidence of laboratory abnormalities based on hematology, clinical chemistry, and urinalysis test results; 12-lead electrocardiogram (ECG) parameters, vital sign measurements, physical examinations, Columbia-Suicide Severity Rating Scale (C-SSRS) questionnaire scores; the PK parameter endpoints, derived from the plasma concentration-time profiles of caffeine on Day 1 administered with placebo and the PK parameter endpoints derived from a single dose of caffeine in participants at steady state CBD following 13 days of CBD, 20 mg/kg twice daily (b.i.d).

[0053] Design: This was a phase 1, open-label, single site trial to investigate the effect of multiple dose administration of CBD on the PK of caffeine in healthy subjects. The duration of the trial was approximately 10 weeks, which includes a screening period (up to 4 weeks), a treatment period (4 weeks) and a safety follow-up period (2 weeks). After signing the informed consent form (ICF), participants entered the screening period (Day −28 to −1). On Day −1, which is the day prior to Day 1, the first day of IMP (caffeine+placebo) administration, screened participants who continued to meet eligibility criteria were admitted to the clinical research unit (CRU). The subjects were resident in the CRU for 2 periods. Subjects were administered a concurrent dose of 7.5 mL of placebo oral solution and 200 mg caffeine on Day 1, 30 minutes after starting a standardized breakfast. They were discharged on Day 3 after completion of the assessments. On Day 3, the first dose of CBD was taken in the morning in the CRU, and on this day, the escalating doses of CBD were dispensed to subjects to be taken at home from Day 4 to Day 12. After discharge on Day 3, the subjects returned to the CRU for ambulatory visits on Days 12, 18, and 23. At these ambulatory visits, the maintenance doses of CBD were dispensed to subjects to be taken at home from Day 13 to Day 25 (the evening dose of Day 25 was taken in the CRU). The subjects were admitted again to the CRU in the afternoon of Day 25. On Days 26 and 27, subjects received CBD b.i.d, and on Day 26, a single oral dose of caffeine was given concurrently with the morning dose of CBD. The subjects were discharged on Day 28 after completion of the assessments. The subjects had a follow-up visit 14 to 16 days after the last IMP dose. In addition to the scheduled follow-up visit, several subjects came back to the CRU after Day 28 for unscheduled visits for additional blood sampling regarding out-of-normal reference range values of liver enzymes. CBD and caffeine were administered as shown in Table 3.

TABLE-US-00003 TABLE 3 Treatment Schedule Day Morning Dose Evening Dose  1 7.5 mL placebo oral Not applicable solution (matched to CBD) 200 mg caffeine oral tablet  3 250 mg CBD: 2.5 mL oral Not applicable solution 4-5 250 mg CBD: 2.5 mL oral 250 mg CBD: 2.5 mL oral solution solution 6-7 500 mg CBD: 5 mL oral 250 mg CBD: 2.5 mL oral solution solution 8-9 500 mg CBD: 5 mL oral 500 mg CBD: 5 mL oral solution solution 10-11 750 mg CBD: 7.5 mL oral 500 mg CBD: 5 mL oral solution solution 12-25 750 mg CBD: 7.5 mL oral 750 mg CBD: 7.5 mL oral solution solution 26 750 mg CBD: 7.5 mL oral 750 mg CBD: 7.5 mL oral solution solution 200 mg caffeine oral tablet 27 750 mg CBD: 7.5 mL oral 750 mg CBD: 7.5 mL oral solution solution

[0054] Formulation Mode of Administration, Dose, Regimen: The CBD formulation is an oral liquid formulation that is clear and colourless to yellow in appearance (100 mg/mL CBD in sesame oil with anhydrous ethanol, added sweetener (sucralose), and strawberry flavouring. The oral liquid formulation is administered with a syringe. The CBD formulation is taken b.i.d. 30 minutes after starting a standard meal. In this trial, a maximum dose of 750 mg CBD b.i.d was selected, considered a therapeutic dose in epilepsy patients.

[0055] The placebo is an oral liquid formulation (sesame oil and anhydrous ethanol with added sweetener [sucralose], and strawberry flavouring). The oral liquid formulation was administered with a syringe.

[0056] The caffeine is provided as a 50 mg tablet.

[0057] On Day 1 and Day 26, the IMP (caffeine and placebo on Day 1, and caffeine and CBD on Day 26) were taken between 08:00 hours and 09:00 hours. From Day 3 to Day 27, the morning dose of CBD was taken approximately at 08:00 h and the evening dose (not applicable on Day 3) was taken 12 hours later. Dosing for each individual subject was to be at around the same time (±1 hour) on each dosing day. The time of the morning dose on Day 26 matched the time of the morning dose on Day 1 (with a margin of ±5 minutes).

[0058] The use of all prescribed medication and all over-the-counter medication, vitamin preparations and other food supplements, or herbal medications was prohibited from first admission to the CRU until the follow-up visit. The use of methylxanthine-containing beverages or food (coffee, [iced] tea, cola, chocolate [milk], mocha drinks/sweets, energy drinks) was not allowed from first admission to the CRU until discharge on Day 28. Foods and beverages containing grapefruit, Seville oranges, pomelos, star fruit, or cranberries, or cruciferous vegetables were not allowed from first admission to the CRU until discharge on Day 28. Alcohol was not allowed from 48 hours prior to each admission to the CRU and throughout the inpatient period, and from 48 hours prior to the safety follow-up visit. Strenuous exercise was not allowed from 7 days prior to first admission to the CRU until the follow-up visit. Subjects were not to consume any foods containing poppy seeds within 72 hours (3 days) prior to each admission to the CRU as this could cause a false positive drug screen result. The use of tobacco- or nicotine-containing products was not allowed from first admission to the CRU until the follow-up visit.

[0059] Pharmacokinetic Assessments: Plasma concentrations of caffeine and its metabolite paraxanthine were determined on the following days: 1, 2, 3, 26, 27 and 28. Plasma concentration of CBD determined on the following days: 23, 25, and 26. These were determined using liquid chromatography and tandem mass spectrometry.

[0060] The following assessments were performed: demographics, medical history, physical examination, C-SSRS, vital signs, body weight, height, 12-lead ECG, adverse events (AEs), previous and concomitant medications recorded. Clinical laboratory samples including chemistry, hematology, serology, urine drug screen, alcohol test.

[0061] Trial subjects were sixteen healthy male and female subjects aged between 18 and 60. All 16 participants took at least 1 dose of trial drug; 9 (56%) completed treatment as planned and received the expected total dose of 400 mg caffeine and 31.25 g cannabidiol.

Results

[0062] Plasma concentrations of caffeine and paraxanthine following administration of caffeine+placebo and of caffeine+CBD are presented in FIGS. 1 and 2.

[0063] Trough plasma samples for CBD were taken on Days 23, 25, and 26. Trough levels of CBD confirmed that CBD had reached steady state before caffeine and CBD were coadministered on Day 26.

[0064] After dosing with 200 mg caffeine and placebo on Day 1 and coadministration of 200 mg caffeine and 750 mg CBD on Day 26, caffeine and its metabolite paraxanthine were quantifiable in the majority of subjects at the first sampling time point, i.e., 0.5 hours.

[0065] On Day 1, following administration of 200 mg caffeine and placebo, maximum postdose geometric mean plasma concentrations were reached at 1.5 hours for caffeine and 6.0 hours for paraxanthine. On Day 26, following coadministration of 200 mg caffeine and 750 mg CBD, maximum postdose geometric mean plasma concentrations were reached at 3.0 hours for caffeine and 14.0 hours for paraxanthine.

[0066] As is apparent from the individual and geometric mean profiles, the elimination phase of caffeine and paraxanthine was multiphasic following 200 mg caffeine and 750 mg CBD coadministration on Day 26, and caffeine concentrations were higher and paraxanthine concentrations lower compared with administration of 200 mg caffeine and placebo on Day 1.

[0067] The PK parameters for caffeine and paraxanthine are presented in Table 4. The differences between geometric mean and individual subject PK parameters for caffeine and paraxanthine following administration of caffeine+placebo (Day 1) and of caffeine+CBD (Day 26) are shown in FIGS. 3 (C.sub.max) and 4 (AUC.sub.0-∞), and the statistical analyses of the differences in PK parameters are presented in Table 5.

TABLE-US-00004 TABLE 4 Summary of the Pharmacokinetic Parameters (Geometric Mean [Geometric CV %]) of Caffeine and Paraxanthine Following Administration of Caffeine + Placebo (Day 1) and of Caffeine + CBD (Day 26) Primary Analysis Sensitivity Analysis Caffeine + Placebo Caffeine + CBD Caffeine + CBD (Day 1) (D 26-FU) (D 26-FU) Parameter (N = 16) (N = 9) (N = 6) Caffeine AUC.sub.0-t (ng .Math. h/mL) 40000 (56.7) 78300 (37.2) 85500 (35.1) AUC.sub.0-∞ (ng .Math. h/mL) 40900 (57.6) 83400 (41.0) 92300 (39.4) C.sub.max (ng/mL) 4600 (23.5) 5170 (21.1) 5430 (19.0) t.sub.max.sup.a (h) 1.51 (0.50-3.00) 3.00 (0.50-5.00) 3.00 (0.50-4.13) Paraxanthine AUC.sub.0-t (ng .Math. h/mL) 21500 (27.8) 23900 (12.8) 23900 (14.0) AUC.sub.0-∞ (ng .Math. h/mL) 23000 (30.2) 27900 (18.4) 28100 (20.1) C.sub.max (ng/mL) 1230 (20.6) 885 (15.8) 894 (17.1) t.sub.max.sup.a (h) 7.99 (4.00-18.02) 14.00 (5.97-18.00) 14.00 (10.00-18.00) FU = follow-up; max = maximum; min = minimum; PK = pharmacokinetic. Note: For the treatment of caffeine + placebo, the primary analysis and sensitivity analysis are equal. .sup.aMedian (min-max).

TABLE-US-00005 TABLE 5 Statistical Analysis of the Pharmacokinetic Parameters of Caffeine and Paraxanthine Following Administration of Caffeine + Placebo (Day 1) and of Caffeine + CBD (Day 26) Ratio Test/Reference Geometric LS Means 90% CI Analyte PK Parameter n Reference n Test Estimate [Lower, Upper] Primary Analysis Caffeine C.sub.max.sup.a (ng/mL) 16 4600 9 5269 1.15 [1.04, 1.26] AUC.sub.0-t.sup.a (ng .Math. h/mL) 16 39969 9 75237 1.88 [1.56, 2.27] AUC.sub.0-∞.sup.a (ng .Math. h/mL) 16 40856 9 79718 1.95 [1.62, 2.35] t.sub.max.sup.b (h) 9 1.52 9 3.00 0.58 [0.01, 1.50] Paraxanthine C.sub.max.sup.a (ng/mL) 16 1227 7 961 0.78 [0.72, 0.86] AUC.sub.0-t.sup.a (ng .Math. h/mL) 16 21454 7 23579 1.10 [0.96, 1.26] AUC.sub.0-∞.sup.a (ng .Math. h/mL) 16 22972 7 27038 1.18 [1.03, 1.35] t.sub.max.sup.b (h) 7 8.00 7 14.00 3.49 [0.48, 6.00] Sensitivity Analysis Caffeine C.sub.max.sup.a (ng/mL) 16 4600 6 5460 1.19 [1.03, 1.36] AUC.sub.0-t.sup.a (ng .Math. h/mL) 16 39969 6 71265 1.78 [1.39, 2.29] AUC.sub.0-∞.sup.a (ng .Math. h/mL) 16 40856 6 76272 1.87 [1.45, 2.41] t.sub.max.sup.b (h) 6 2.25 6 3.00 0.57 [0.00, 1.25] Paraxanthine C.sub.max.sup.a (ng/mL) 16 1227 6 984 0.80 [0.73, 0.88] AUC.sub.0-t.sup.a (ng .Math. h/mL) 16 21454 6 22526 1.05 [0.93, 1.18] AUC.sub.0-∞.sup.a (ng .Math. h/mL) 16 22972 6 26023 1.13 [0.99, 1.30] t.sub.max.sup.b (h) 6 8.00 6 14.00 3.99 [−0.02, 7.00]  CI = confidence interval; LS = least squares; PK = pharmacokinetic. Note: Reference, caffeine + placebo treatment; Test, caffeine + CBD treatment. .sup.aAUC and C.sub.max, the interaction effect was explored using a mixed effect (analysis of variance) model with treatment as fixed factor and subject as a random effect. .sup.bt.sub.max, nonparametric Wilcoxon signed-rank test presenting the Hodges-Lehman estimate and 90% CI based on the Tukey method. Median, median of the difference, and approximate 90% CI for the difference are presented.

[0068] For caffeine, as shown by the point estimates for the treatment ratios (primary analysis) in Table 5, when compared with caffeine and placebo (Day 1), coadministration of caffeine and CBD (Day 26) resulted in a slight increase in C.sub.max (1.15, 90% CI: [1.04, 1.26]) and a larger increase in AUC.sub.0-t (1.88, 90% CI: [1.56, 2.27]) and AUC.sub.0-∞ (1.95, 90% CI: [1.62, 2.35]). The t.sub.max for caffeine was later after administration of caffeine and CBD (Day 26) compared with caffeine and placebo administration (Day 1) (difference Hodges-Lehman estimate: 0.58, 90% CI: [0.01, 1.50]).

[0069] For paraxanthine, as shown by the point estimates for the treatment ratios (primary analysis), when compared with caffeine and placebo (Day 1), coadministration of caffeine and CBD (Day 26) resulted in a decrease in C.sub.max (0.78, 90% CI: [0.72, 0.86]) and a slight increase in AUC.sub.0-t (1.10, 90% CI: [0.96, 1.26]) and AUC.sub.0-∞ (1.18, 90% CI: [1.03, 1.35]). The t.sub.max for paraxanthine tended to be later after administration of caffeine and CBD (Day 26) compared with caffeine and placebo administration (Day 1) (difference Hodges-Lehman estimate: 3.49, 90% CI: [0.48, 6.00]).

[0070] Similar results were seen for the primary and sensitivity analyses.

[0071] Thus, exposure to caffeine increased by 15% for C.sub.max and 95% for AUC.sub.0-∞ when caffeine was given with steady-state CBD compared to when caffeine was given with placebo.

[0072] Exposure to the CYP1A2-mediated caffeine metabolite paraxanthine was impacted by CBD coadministration as evidenced by a 22% decrease in C.sub.max and 18% increase in AUC.sub.0-∞. The t.sub.max for paraxanthine was delayed when caffeine was coadministered with CBD, which may reflect a slower formation of the metabolite.

[0073] FIG. 5 provides a visual summary of the results of the primary PK endpoint for the trial, illustrating the point estimates for the ratio of the geometric LS means and the 90% CI for exposure to caffeine and paraxanthine when subjects were administered caffeine in the presence of steady-state CBD compared with administration of caffeine and placebo.

[0074] Coadministration of caffeine and CBD resulted in a change in caffeine and paraxanthine exposure (based on AUC.sub.0-t, AUC.sub.0-∞, and C.sub.max). AUC.sub.0-t was increased by 88% and 10% for caffeine and paraxanthine, respectively; AUC.sub.0-∞ was increased by 95% and 18% for caffeine and paraxanthine, respectively; and C.sub.max was increased by 15% and decreased by 22% for caffeine and paraxanthine, respectively, when compared to administration of caffeine and placebo. Taken all together, CBD affects exposure of caffeine and its metabolite paraxanthine.

Conclusions

[0075] Such findings delineate an important concern for epilepsy patients and also for the wider community with the increasing legalization of marijuana. This drug-drug interaction may have implications in epilepsy patients which are not correctly monitored over the course of their treatment.

[0076] Patients that are taking caffeine-containing drugs or products should be carefully monitored over the course of their treatment with CBD to ensure toxicity from prolonged caffeine exposure does not occur.

EXAMPLE 2: LIVER SAFETY

[0077] In the above-outlined Phase 1 trial, abnormal liver chemistries were found for the subjects. This was unexpected as subjects were healthy adults receiving therapeutic equivalent doses of CBD used to treat Dravet Syndrome and Lennox-Gastaut Syndrome (1500 mg/day).

[0078] Measurements were performed at screening, on trial Days −1, 12, 18, 23, 27, and at follow-up.

Results

[0079] The most notable biochemical abnormalities were elevation in serum ALT, the related enzyme AST, and GGT. In 7 (44%) participants, peak serum ALT values were >ULN; in 6 (38%) participants the value was >2×ULN; and in 5 (31%) participants the peak ALT value was >5×ULN, the international consensus criteria for DILI (Table 6). The serial liver chemistries observed in the 5 participants with peak ALT values >5×ULN are displayed in FIG. 6.

[0080] All elevations occurred between 2-4 weeks exposure to cannabidiol, between days 18-27. Among the 6 participants with ALT elevations who were discontinued from the protocol, some had symptoms consistent with hepatitis, fever, or eosinophilia.

TABLE-US-00006 TABLE 6 Observed peak serum ALT and fold-changes from baseline value Reference ULN >ULN ≥2 × ULN ≥3 × ULN ≥5 × ULN ≥10 × ULN ≥20 × ULN Stated ULN 7 (44%) 6 (38%) 5 (31%) 5 (31%) 0 (0) 0 (0)

Conclusions

[0081] Therapeutic doses of cannabidiol administered to healthy adults can result in elevations in serum alanine aminotransferase consistent with drug-induced liver injury. Physicians should be alert to this potential effect from cannabidiol and be on the lookout for association with clinically important liver injury.

[0082] Furthermore, abnormal liver chemistries in healthy volunteers dosed with CBD at the doses used in this study have not heretofore been observed at the high rates seen in this trial (44%). As such the DDI observed between CBD and caffeine may have an impact on the DILI experienced by these patients.

[0083] It is therefore imperative that levels of CBD, caffeine, and liver enzymes (ALT, AST, and GGT) are measured in patients administered CBD who are concurrently taking caffeine either as a medication or recreationally. Caution is required to ensure DILI does not occur in these patients. Reduction of the dose of CBD, the dose of caffeine or the doses of both CBD and caffeine may be required to ensure patients liver chemistries are safe.

REFERENCES

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